Novel Gold-Based Nanocrystals for Medical Treatments and Electrochemical Manufacturing Processes Therefor
20210361699 · 2021-11-25
Assignee
Inventors
- Mark Gordon Mortenson (North East, MD)
- D. Kyle Pierce (Elkton, MD)
- David A. Bryce (Elkton, MD)
- Reed N. Wilcox (Littleton, CO)
- Anthony Lockett (Leeds, GB)
- Mikhail Merzliakov (Parkville, MD)
Cpc classification
A61P1/04
HUMAN NECESSITIES
A61P29/00
HUMAN NECESSITIES
A61P9/10
HUMAN NECESSITIES
B22F1/0553
PERFORMING OPERATIONS; TRANSPORTING
A61K9/0095
HUMAN NECESSITIES
A61P19/06
HUMAN NECESSITIES
B22F1/0545
PERFORMING OPERATIONS; TRANSPORTING
B22F9/00
PERFORMING OPERATIONS; TRANSPORTING
A61P1/16
HUMAN NECESSITIES
A61P35/00
HUMAN NECESSITIES
A61P25/14
HUMAN NECESSITIES
Y02A50/30
GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
A61P21/00
HUMAN NECESSITIES
A61P25/28
HUMAN NECESSITIES
B82Y30/00
PERFORMING OPERATIONS; TRANSPORTING
A61P37/06
HUMAN NECESSITIES
A61K9/14
HUMAN NECESSITIES
International classification
A61K9/00
HUMAN NECESSITIES
A61K9/14
HUMAN NECESSITIES
B22F1/00
PERFORMING OPERATIONS; TRANSPORTING
B22F9/00
PERFORMING OPERATIONS; TRANSPORTING
B82Y30/00
PERFORMING OPERATIONS; TRANSPORTING
Abstract
The present invention relates to novel gold nanocrystals and nanocrystal shape distributions that have surfaces that are substantially free from organic impurities or films. Specifically, the surfaces are “clean” relative to the surfaces of gold nanoparticles made using chemical reduction processes that require organic reductants and/or surfactants to grow gold nanoparticles from gold ions in solution.
The invention includes novel electrochemical manufacturing apparatuses and techniques for making the gold-based nanocrystals. The invention further includes pharmaceutical compositions thereof and the use of the gold nanocrystals or suspensions or colloids thereof for the treatment or prevention of diseases or conditions for which gold therapy is already known and more generally for conditions resulting from pathological cellular activation, such as inflammatory (including chronic inflammatory) conditions, autoimmune conditions, hypersensitivity reactions and/or cancerous diseases or conditions. In one embodiment, the condition is mediated by MT (macrophage migration inhibiting factor).
Claims
1. A method for treating a patient with amyotrophic lateral sclerosis disease, comprising administering to a patient in need thereof an effective amount of a pharmaceutically acceptable suspension comprising: a.) pharmaceutical grade water; b.) at least one processing enhancer comprising sodium bicarbonate; c.) gold nanocrystals suspended in said water forming a suspension, wherein said gold nanocrystals: i.) have surfaces that do not have organic chemical constituents adhered or attached to said surfaces: ii.) have a mode particle size of less than about 50 nm; iii.) are present in said suspension at a concentration of at least 2 ppm; and d.) said suspension having a pH of between about 5 to about 9.5, said gold nanocrystals having a zeta potential of about −20 my or lower at a temperature of about 25′C, said zeta potential being determined by measuring the electrophoretic mobility of the gold nanocrystals in the suspension, and the suspension does not contain chloride ions.
2. The method of claim 1, wherein said suspension is administered orally.
3. A method for treating a patient with amyotrophic lateral sclerosis disease, comprising administering to a patient in need thereof an effective amount of a pharmaceutically acceptable suspension comprising: a.) water; b.) at least one processing enhancer; c.) gold nanocrystals suspended in said water forming a suspension, wherein said gold nanocrystals: i) have surfaces that do not have organic chemical constituents adhered or attached to said surfaces; ii.) have a mode particle size of less than about 50 nm; iii.) are present in said suspension at a concentration of at least 2 ppm; and d.) said suspension having a pH of between about 5 to about 9.5, said gold nanocrystals having a zeta potential of about −20 my or lower at a temperature of about 25° C., said zeta potential being determined by measuring the electrophoretic mobility of the gold nanocrystals in the suspension.
4. The method of claim 3, wherein said suspension is administered orally.
5. A method for treating a patient with amyotrophic lateral sclerosis disease, comprising administering to a patient in need thereof an effective amount of a pharmaceutical suspension comprising: a.) water and sodium bicarbonate dissolved therein, said suspension medium having a pH of between about 5 to about 9.5; b.) shaped gold nanocrystals in said suspension medium forming a suspension, said shaped gold nanocrystals having a zeta potential of about −30 mV or lower at a temperature of about 25° C., said zeta potential being determined by measuring the electrophoretic mobility of the shaped gold nanocrystals in the pharmaceutical suspension; and wherein said shaped gold nanocrystals: i.) have surfaces that do not have organic chemical constituents adhered or attached to said surfaces: ii.) have a mode particle size of less than about 30 nm; iii.) are present in said suspension at a concentration of at least about 2 ppm; and iv.) comprise triangle and pentagon shapes.
6. The method of claim 5, wherein said suspension is administered orally.
7. The method of claim 1, wherein said gold nanocrystals have a zeta potential of about −30 mV or lower.
8. The method of claim 1, wherein said gold nanocrystals have a zeta potential of about −40 mV or lower.
9. The method of claim 1, wherein said gold nanocrystals have a zeta potential of about −50 mV or lower.
10. The method of claim 1, wherein said gold nanocrystals have shapes comprising faces with spatially extended low index crystal planes, said shapes appearing as triangles and pentagons when dried from suspension on a surface.
11. The method of claim 10, wherein said shaped gold nanocrystals further comprise shapes which appear as hexagons and diamond shapes when dried from suspension on a surface.
12. The method of claim 1, wherein said gold nanocrystals are present at a concentration of about 2-200 ppm.
13. The method of claim 1, wherein said mode particle size is within a range of about 8-18 nm and said pH is between about 8 to about 9.5.
14. The method of claim 13, wherein said gold nanocrystals are shaped and have low Miller index crystal planes arranged into shapes comprising triangles and pentagons.
15. The method of claim 14, wherein said shaped gold nanocrystals having said low Miller index crystal planes further comprise shapes of hexagons and diamonds.
16. The method of claim 1, wherein said gold nanocrystals are shaped and include at least one low Miller index crystal plane selected from the group of crystal planes consisting of {111}, {110} and {100}.
17. The method of claim 1, wherein said gold nanocrystals are shaped and comprise at least one low Miller index {111} crystal plane.
18. The method of claim 1, wherein said gold nanocrystals have a mode particle size of less than about 30 nm.
19. The method of claim 1, wherein said gold nanocrystals have a mode particle size within a range of about 8-18 nm.
20. The method of claim 3, wherein said gold nanocrystals are present at a concentration of about 2-200 ppm.
21. The method of claim 5, wherein said gold nanocrystals are present at a concentration of about 2-200 ppm.
22. The method of claim 3, wherein said at least one processing enhancer comprises at least one material selected from the group of materials consisting of sodium bicarbonate, sodium carbonate, potassium bicarbonate, potassium carbonate, trisodium phosphate, disodium phosphate, monosodium phosphate, potassium phosphates or other salts of carbonic acid.
23. The method of claim 3, wherein said suspension does not contain chloride ions.
24. A method for treating a patient with amyotrophic lateral sclerosis disease comprising administering orally to a patient in need thereof an effective amount of a pharmaceutically acceptable suspension comprising: a.) water and NaHCO.sub.3 dissolved therein; b.) gold nanocrystals suspended in said water forming a suspension, wherein said gold nanocrystals: i.) have surfaces that do not have organic chemical constituents adhered or attached to said surfaces; ii.) have a mode particle size of less than about 50 nm; iii.) are present in said pharmaceutical suspension at a concentration of at least 2 ppm iv.) are shaped and comprise at least one low Miller index crystal plane selected from the group of crystal planes consisting of {111}, {110} and {100}; and c.) said suspension having a pH of between about 8 to about 9.5, said gold nanocrystals have a zeta potential of about −30 mV or lower at a temperature of about 25° C., said zeta potential being determined by measuring the electrophoretic mobility of the gold nanocrystals in the pharmaceutical suspension, and the pharmaceutical suspension does not contain chloride ions.
25. The method of claim 24, wherein said gold nanocrystals have shapes comprising faces with spatially extended low index crystal planes, said shapes appearing as triangles and pentagons when dried from suspension on a surface.
26. The method of claim 25, wherein said shaped gold nanocrystals further comprise hexagon and diamond shapes.
27. The method of claim 24, wherein said at least one low Miller index crystal plane comprises a crystal plane {111}.
Description
BRIEF DESCRIPTION OF THE FIGURES
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DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS
[0288] I. Novel Gold Nanocrystals
[0289] New gold nanocrystals are provided that have nanocrystalline surfaces that are substantially free from organic or other impurities or films. Specifically, the surfaces are “clean” relative to those made using chemical reduction processes that require chemical reductants and/or surfactants to form gold nanoparticles from gold ions in solution. The new gold nanocrystals are produced via novel manufacturing procedures, described in detail herein. The new manufacturing procedures avoid the prior use of added chemical reductants and/or surfactants (e.g., organic compounds) or other agents which are typically carried along in, or on, the particles or are coated on the surface of the chemically reduced particles; or the reductants are subsequently stripped or removed using undesirable processes which themselves affect the particle.
[0290] In a preferred embodiment, the process involves the nucleation and growth of the gold nanocrystals in water which contains a “process enhancer” or “processing enhancer” (typically an inorganic material or carbonate or such) which does not significantly bind to the formed nanocrystals, but rather facilitates nucleation/growth during electrochemical-stimulated growth process. The process enhancer serves important roles in the process including providing charged ions in the electrochemical solution to permit the crystals to be grown. The process enhancer is critically a compound(s) which remains in solution, and/or does not form a coating (e.g., an organic coating), and/or does not adversely affect the formed nanocrystals or the formed suspension(s), and/or is destroyed, evaporated, or is otherwise lost during the electrochemical process. A preferred process enhancer is sodium bicarbonate. Examples of other process enhancers are sodium carbonate, potassium bicarbonate, potassium carbonate, trisodium phosphate, disodium phosphate, monosodium phosphate, potassium phosphates or other salts of carbonic acid or the like. Further process enhancers may be salts, including sodium or potassium, of bisulfite or sulfite. Still other process enhancers to make gold nanocrystals for medical applications under certain conditions may be other salts, including sodium or potassium, or any material that assists in the electrochemical growth processes described herein; which is not substantially incorporated into or onto the surface of the gold nanocrystals; and does not impart toxicity to the nanocrystals or to the suspension containing the nanocrystals.
[0291] Desirable concentration ranges for the processing enhancer include typically 0.01-20 grams/gallon (0.0026-2.1730 mg/ml), more typically, 0.1-7.5 grams/gallon (0.0264-1.9813 mg/ml) and most typically, 0.5-2.0 grams/gallon (0.13210-0.5283 mg/ml).
[0292] Because the grown gold nanocrystals have “bare” or “clean” surfaces of gold metal (e.g., in the zero-oxidation state) the surfaces are highly reactive or are highly biocatalytic (as well as highly bioavailable). The nanocrystals are essentially surrounded by a water jacket. These features provide increased efficacy in vivo relative to nanoparticle surfaces that contain, for example, organic material present from reduction chemistry processes. The “clean” surfaces may also reduce the toxicity of the nanocrystals, over those nanoparticles that contain coated or “dressed” surfaces. The increased efficacy of these “clean” gold nanocrystals may provide an increased therapeutic index via a lower dose needed to achieve a therapeutic effect. A comparative mouse model example herein (Example 25) compares an inventive gold nanocrystal suspension to Auranofin, a commercially available and FDA-approved gold drug, This Example shows that these novel gold nanocrystals, in mice, are at least 5 times more active than Auranofin in the well-accepted collagen induced arthritis model of inflammation in rheumatoid arthritis.
[0293] Specifically, the comparative mouse model (Example 25) compares the dose levels demonstrating efficacy using an inventive crystal suspension to the dose levels demonstrating efficacy using Auranofin, a commercially available and FDA-approved gold-based drug, Example 25 shows that these novel gold nanocrystals, in mice, achieve efficacy at a dose level at least 17 times lower than the effective dose level of Auranofin in the well accepted collagen induced arthritis model of inflammation in the mouse, and 5 times lower than the gold content contained in the effective dose level of Auranofin. Thus, comparing relative efficacy levels of the novel gold nanocrystal to those of the gold-based drug Auranofin, and to only the gold content of those of the Auranofin, the relative potency of the novel gold nanocrystals is 17 times greater than Auranofin and 5 times greater than the gold contained in the Auranofin.
[0294] This potency advantage means that treatment efficacy can be achieved at a much lower dose level (17× lower dose than Auranofin, 5× lower dose than the gold contained in Auranofin), or alternatively, that potentially much greater efficacy can be achieved at equivalent dose levels.
[0295] There are other important advantages of the novel nanocrystals in two other dimensions: relative toxicity, and relative speed of onset of benefits. With respect to both observed relative toxicity, and observed relative speed of onset of benefits, in an animal model, the novel gold nanocrystals are significantly different and significantly outperform Auranofin, the only orally administrated, FDA-approved gold-based pharmaceutical product in the prior art.
[0296] In a preferred embodiment, the nanocrystals are not dried before use but instead used in the liquid they were formed in (i.e., forming a suspension) or a concentrate or a reconstituted concentrate thereof. It appears that completely removing these crystals from their suspension (e.g., completely drying) may, in certain cases, affect the surface properties of the crystals, (e.g., partial oxidation may occur) and/or may affect the ability to rehydrate the crystals by, for example, altering the initially formed water jacket. This suggests that it may be optimal to use sterile pharmaceutical grade water (i.e., USP) and the aforementioned process enhancers in the manufacturing processes.
[0297] The gold nanocrystals made according to this invention can also be used for industrial applications where gold reactivity is important (e.g., catalytic and/or electrochemical processes) but pharmaceutical grade products are not required. When prepared for non-pharmaceutical uses, the gold nanocrystals can be made in a wider variety of solvents and with a wider variety of process enhancers, depending on the application.
[0298] According to the processes herein, the gold nanocrystals can be grown in a manner that provides unique and identifiable surface characteristics such as spatially extended low index, crystal planes {111}, {110} and/or {100} and groups of such planes (and their equivalents). The shapes of the gold nanocrystals prepared according to the processes described herein include, but are not limited to, triangles (e.g., tetrahedrons), pentagons (e.g., pentagonal bipyramids or decahedrons), hexagons (e.g., hexagonal bipyramids, icosahedrons, octahedrons), diamond (e.g., octahedrons, various elongated bipyramids, fused tetrahedrons, side views of bipyramids) and “others”. The percent of nanocrystals (i.e., grown by various embodiments set forth herein) containing the aforementioned spatially extended low index crystal planes and having “clean” surfaces is another novel feature of the invention. Furthermore, the percent of tetrahedrons and/or pentagonal bipyramids formed or present in the nanocrystalline suspensions is/are also unique.
[0299] In a preferred embodiment the percent of pentagonal bipyramids is at least about 5%, or is in a range of about 5%-35%, and more typically at least about 10%, or is in a range of about 10%-35%, and even more typically, at least about 15%, or is in a range of about 15%-35%, and still more typically, at least about 25%, and in some cases at least about 30%.
[0300] In another preferred embodiment the percent of tetrahedrons is at least 5%, or is in a range of about 5%-35%, and more typically at least about 10%, or is in a range of about 10%-35%, and even more typically, at least about 15%, or is in a range of about 15%-35%, and still more typically, at least about 25%, and in some cases at least about 30%.
[0301] Still further, the combination of pentagonal bipyramids and tetrahedrons is at least about 15%, or is in a range of about 15%-50%, and more typically at least about 20%, or is in a range of about 20%-50%, and even more typically, at least about 30%, or is in a range of about 30%-50%, and still more typically, at least about 35%, and in some cases at least about 45%.
[0302] Still further, the combination of pentagonal bipyramids, tetrahedrons, octahedrons and hexagonal is at least about 50%, or is in a range of about 50%-85%, and more typically at least about 60%, or is in a range of about 60%-85%, and even more typically, at least about 70%, or is in a range of about 70%-85%, and still more typically, at least about 70%, and in some cases at least about 80%.
[0303] Any desired average size of gold nanocrystals below 100 nm can be provided. The most desirable crystalline size ranges include those having an average crystal size or “mode” (as measured and determined by specific techniques disclosed in detail herein and reported as “TEM average diameter”) that is predominantly less than 100 nm, and more typically less than 50 nm, even more typically less than 30 nm, and in many of the preferred embodiments disclosed herein, the mode for the nanocrystal size distribution is less than 21 nm and within an even more preferable range of 8-18 nm.
[0304] Resulting gold nanocrystalline suspensions or colloids can be provided that have or are adjusted to have target pH ranges. When prepared with, for example, a sodium bicarbonate process enhancer, in the amounts disclosed in detail herein, the pH range is typically 8-9, which can be adjusted as desired.
[0305] The nature and/or amount of the surface change (i.e., positive or negative) on formed nanoparticles or nanocrystals can have a large influence on the behavior and/or effects of the nanoparticle/suspension or colloid. For example, protein coronas such as albumin coronas formed in vivo can be influenced by surface charge or surface characteristics of a nanoparticle. Such surface charges are commonly referred to as “zeta potential”. It is known that the larger the zeta potential (either positive or negative), the greater the stability of the nanoparticles in the solution (i.e., the suspension is more stable). By controlling the nature and/or amount of the surface charges of formed nanoparticles or nanocrystals, the performance of such nanoparticle suspensions can be controlled.
[0306] Zeta potential is known as a measure of the electro-kinetic potential in colloidal systems and is also referred to as surface charge on particles. Zeta potential is the potential difference that exists between the stationary layer of fluid and the fluid within which the particle is dispersed. A zeta potential is often measured in millivolts (i.e., mV). The zeta potential value of approximately 20-25 mV is an arbitrary value that has been chosen to determine whether or not a dispersed particle is stable in a dispersion medium. Thus, when reference is made herein to “zeta potential”, it should be understood that the zeta potential referred to is a description or quantification of the magnitude of the electrical charge present at the double layer.
[0307] The zeta potential is calculated from the electrophoretic mobility by the Henry equation:
where z is the zeta potential, U.sub.E is the electrophoretic mobility, ε is a dielectric constant, η is a viscosity, f(ka) is Henry's function. For Smoluchowski approximation f(ka)=1.5.
[0308] Zeta potentials (“ZP”) for the gold nanocrystals prepared according the methods herein typically have a ZP of at least −20 mV, more typically at least about −30 mV, even more typically, at least about −40 mV and even more typically at least about −50 mV.
[0309] II. Use of Novel Gold Nanocrystals
[0310] The gold nanocrystals of the present invention can be used to treat any disorder for which gold therapy is known to be effective, which includes a broad range of inflammatory and autoimmune disorders as well as certain infectious diseases and cancer. Descriptions of many of these uses are provided in the Background of the Invention, above, or otherwise, in more detail below.
[0311] The subject to be treated may be human or another animal such as a mammal. Non-human subjects include, but are not limited to primates, livestock animals (e.g., sheep, cows, horses, pigs, goats), domestic animals (e.g., dogs, cats), birds and other animals (e.g., mice, rats, guinea pigs, rabbits).
[0312] Importantly, it has now been surprisingly discovered as part of this invention that the gold nanoparticles (and in particular the gold nanocrystals described in detail herein) inhibit macrophage Migration Inhibitory Factor (“MIF”). It is believed that this is the first disclosure of such activity of gold nanoparticles, and may provide a scientific basis to understand the range of medical uses for gold compositions to date. It also provides a scientific basis to conclude that the gold nanoparticles will be effective against other diseases which are mediated by macrophage migration inhibitory factor. In addition, it has been identified that these gold nanocrystals inhibit IL-6 but not IL-10. Because MIF and/or IL-6 is/are indicated in a large variety of conditions and/or biological signaling pathways, such finding confirms that the novel gold nanocrystals will be effective for the treatment or prevention of diseases or conditions resulting from pathological cellular activation, such as inflammatory (including chronic inflammatory) conditions, autoimmune conditions, certain infections, hypersensitivity reactions and/or cancerous diseases or conditions.
[0313] MIF is a macrophage derived multifunctional cytokine important in a number of pro-inflammatory events. MIF was originally described as a product of activated T-lymphocytes that inhibits the random migration of macrophages. While MIF was initially found to activate macrophages at inflammatory sites, MIF has now been shown to mediate a range of signaling agents in the immune system. MIF has been shown to be expressed in human and animal diseases or conditions which include infection, inflammation, injury, ischemia and/or malignancy. MIF appears to have a key role in cell proliferation, cell differentiation, angiogenesis and wound healing. MIF also seems to mediate glucocorticoid (steroids) activity by counteracting at least some of their anti-inflammatory effects.
[0314] As shown in Examples 25 and 26, the nanocrystalline compositions of the present invention are very effective in the animal models for CIA and EAE. A connection between these two animal models (as well as human disease state) is the presence of MIF.
[0315] Recent studies have indicated that monoclonal antibody antagonism of MIF may be useful in the treatment of sepsis, certain types of cancers and delayed type hypersensitivity. It appears that sepsis is triggered by an over-reaction of the inflammation and immune systems. In certain infections, upon attack by microorganisms, the innate immune system reacts first, whereby neutrophils, macrophages and natural killer cells (“NK cells”) are mobilized. Cytokines (and MIF) thus play an important role as mediators, which regulate activation and differentiation of these cells. Finally, the innate immune system interacts with the adaptive immune system via these and other stimulating molecules, upon which the adaptive immune system has the ability of constructing an immunological memory in addition to providing pathogen specific protection.
[0316] MIF is seen as a major mediator in sepsis, as MIF incites the production of TNF, other pro-inflammatory cytokines and eicosanoids, induces the expression of TLR-4, which recognizes LPS, and appears to resist in activating the innate immune response. MIF and glucocorticoids act as antagonists and are at least partially responsible for regulating the inflammatory reaction. MIF has an inhibiting effect on glucocorticoids, which typically inhibit inflammation.
[0317] Therapeutic antagonism of MIF can provide “steroid-sparing” effects or can even be therapeutic in “steroid-resistant” diseases. Unlike other pro-inflammatory molecules, such as certain cytokines, the expression and/or release of MIF is coupled to (e.g., can be induced by) glucocorticoids. MIF seems to be able to antagonize the effects of glucocorticoids. MIF has a major role in regulating pro-inflammatory cytokines. This has been shown to be the case for macrophages secreting TNF, IL-1.beta., IL-6 and IL-8. MIF also regulates IL-2 release. MIF also has a role in regulating T cell proliferation. In vivo, MIF exerts a powerful glucocorticoid-antagonist effect in models including endotoxic shock and experimental arthritis (e.g., collagen-induced arthritis or “CIA” models, such as the one utilized in a later example herein and models of other inflammatory conditions and immune diseases including colitis, multiple sclerosis (i.e., the EAE model discussed in greater detail in Example 26), atherosclerosis, glomerulonephritis, uveitis and certain cancers).
[0318] Further, MIF has recently been shown to be important in the control of leukocyte-endothelial interactions. Leukocytes interact with vascular endothelial cells in order to gain egress from the vasculature into tissues. The role of MIF in these processes has been demonstrated to affect leukocyte-endothelial adhesion and migration. These processes seem to be an essential part of nearly all inflammatory diseases, and also for diseases less well-identified as inflammatory including, for example, atherosclerosis.
[0319] MIF is also expressed in plants (thus “MIF” may also refer to plant MIF) and where appropriate, the inventive gold nanocrystal suspensions (e.g., comprising aqueous gold-based metal nanocrystals and/or mixtures of gold nanocrystals and other metal(s) and/or alloys of gold nanocrystals with other metal(s) and/or a combination therapy approach) may be used in botanical/agricultural applications such as crop control.
[0320] MIF is a key cytokine in switching the nature of the immune response. The immune response has two effector mechanisms. The Th1 immune response generates cytotoxic T cells that kill pathogens and damaged/defunct cells. The Th2 response generates antibodies that facilitate phagocytosis and activate complement. The role of MIF in determining the polarization of the immune system is dependent on other cytokines such as IL-10. IL-10 is a potent anti-inflammatory cytokine that blocks the action of MIF on Th1 cells and leads to the generation of a Th2 response. In the absence of IL-10 MIF will stimulate Th1 cells to produce a cytotoxic response. IL10 is produced by Monocytes and B cells in response to stimulation, whereas MIF is, for example, independently produced and stored in the pituitary and T cells. MIF therefore plays an important role in both T Cytotoxic cell mediated diseases—such as rheumatoid arthritis and Crohns, and antibody mediated diseases such as idiopathic thrombocytopenia.
[0321] Without wishing to be bound by any particular theory or explanation, when reference is made herein to “one or more signaling pathway(s)” it should be understood as meaning that MIF, or at least one protein associated with MIF (e.g., including receptor sites such as CD74 receptor sites) is/are implicated in the innate immune system (e.g., NK and phagocyte cells, complement proteins (e.g., C5a) and/or inflammatory pathways) and the adaptive immune systems (e.g., the T cell dependent cytotoxicity (Th1) and antibody (Th2) pathways). For example, when MIF is involved in the Th1 signaling pathway generating T Cytotoxic cells other proteins such as, for example, IL6, TNF, and other cytokines are also involved.
[0322] When the Th1 signaling pathway is overactive, a variety of diseases can result, such as rheumatic diseases, connective tissue diseases, vasculitides, inflammatory conditions, vascular diseases, ocular diseases, pulmonary diseases, cancers, renal diseases, nervous system disorders, complications of infective disorders, allergic diseases, bone diseases, skin diseases, Type 1 Diabetes, Crohn's Disease, MS and gastrointestinal diseases, etc. Accordingly, by reducing the amount of MIF function associated with this particular Th1 signaling pathway, chronic disease conditions can be mitigated.
[0323] In contrast, again without wishing to be bound by any particular theory or explanation, when the Th2 signaling pathway is over-active, the production of various antibodies occurs leading to diseases such as, for example and including, hemolytic anemia, ITP (Idiopathic Thrombocytopenic Purpura), Hemolytic Disease of the newborn, etc. Furthermore, over-activity of this Th2 signaling pathway can result in an under-activity of the Th1 pathway, thus permitting various parasites or cancers to thrive. For example, in the case of malaria where over production of one or more homologues of MIF leads to the generation of an ineffective antibody response that is ineffective against the parasite (e.g., it is plausible that a variety of crystal forms or homologues of MIF (or equivalents thereto) are made or presented by a variety of bacteria, parasites, virus, fungi, etc., each of which may have different reactivity relative to, for example, “ordinary” human MIF, and which may alter host immune response so as to create at least local environments of “immune privilege”). Accordingly, by reducing the amount of MIF function associated with this particular Th2 signaling pathway, other disease conditions can be mitigated.
[0324] Still further, without wishing to be bound by any particular theory or explanation, MIF also has a role in driving the signaling pathway associated with innate immunity. This pathway involves the activation of natural killer (“NK”) cells, phagocytes and other non-specific pathogen cell types and certain proteins such as complement proteins (e.g., C5a). Excess MIF (and/or MIF homologues), or similar effects of the same, can result in undesirable over-expression or over-reaction in this particular signaling pathway as seen in multiple organ failure as a result of sepsis. Examples include the Systemic Inflammatory Response Syndrome (SIRS). Accordingly, by reducing the amount of MIF activity associated with this particular signaling pathway many inflammatory diseases can be mitigated.
[0325] Accordingly when endogenous MIF is present (e.g., in excess under local environmental conditions), as measured by, for example, known body fluid measuring techniques such as ELISA, spectroscopy, etc., it is possible that one or more innate or adaptive immune system signaling pathways may over-express, over activate or over-produce inflammatory/immunological components. If for example, one or more forms of MIF present causes the production of an excessive T Cytotoxic response, or an excessive antibody response or an exaggerated NK/phagocyte cell response, human disease can result. When, for example, too many T Cytotoxic cells are expressed, a variety of chronic inflammatory conditions can result. Similarly when excessive Th2 or innate responses are facilitated by MIF, other diseases are produced.
[0326] Still further, it is also known that malaria parasites, and other parasites such as nematodes and filarial worms, and some cancers produce certain types of exogenous or non-regulated MIF or MIF homologues. Again, without wishing to be bound by any particular theory or explanation, it appears that exogenous expression of MIF, or its homologues, leads to stimulation of the Th2 signaling pathway, and may be an attempt by the parasite, or the tumor, (i.e., “the invader”) to create a state where the immune response is activated by MIF or its homologues such that that the activated particular signaling pathway is not detrimental to the tumor or the parasite, etc.
[0327] With regard to, for example, a malaria parasite, the parasite may stimulate the Th2 signaling pathway by providing excess exogenous MIF resulting in the production of antibodies rather than T Cytotoxic cells. However, such antibodies do not typically harm the parasite. Therefore, the parasite appears to create at least a local area of immune privilege. In this regard if an alternative pathway such as, for example, the Th1 pathway, or the natural killer (NK) cell pathway, can be re-activated, damage could then occur to the parasite (e.g., the immune system could remove the parasite). However, if excess antibodies or other immune/inflammatory products are created, for example, as a result of the preferential activation of the Th2 pathway, it is possible that the excess antibodies will end up cross-linking to various cell sites or activating other immunological molecules. When such cross-linking or activation occurs, a very large inflammatory response could result. Without wishing to be bound by any particular theory or explanation, it is possible that this inflammatory response is precisely the response that occurs in women who are pregnant and are infected with malaria making them vulnerable to severe malaria, and the anemia of malaria. It is believed that pregnant women are particularly susceptible to this effect, due to the immunological effects of the placenta in promoting a Th2 response and sequestering parasites in this immune-privileged zone.
[0328] Again, without wishing to be bound by any particular theory or explanation, cancer cells also express MIF apparently in an attempt to at least partially control immune response thereto and/or promote their own growth. In this regard, it appears that cancer cells are also attempting to manipulate the immune system to follow the Th2 signaling pathway, in contrast to the Th1 signaling pathway which could damage or kill the cancer cells. For example, by causing local immune privilege to be created, there is no (or little) particular risk to cancer cells. In contrast, if MIF was to stimulate the Th1 signaling pathway, then a cytokine cell/inflammatory response may result, causing damage or death to the cancer cells (e.g., the tumor could be naturally eliminated by the immune system).
[0329] Again, without wishing to be bound by any particular theory or explanation, children possess an immature immune system, particularly the innate and Th1 pathways. This immaturity in some children results in altered MIF metabolism. It thus appears that the modulation of MIF in children could result in the prevention or improvement of infectious or inflammatory diseases.
[0330] Accordingly, without wishing to be bound by any particular theory or explanation, the inventive gold nanocrystal suspensions of the present invention can be used to modify one or more signaling pathways (e.g., Th1 signaling pathway, Th2 signaling pathway and/or innate immunity pathway) either alone or in conjunction with other therapies that modulate signaling pathways. Thus, by interacting with or controlling the MIF (or MIF homologue) associated with one or more signaling pathway(s), various immunological responses can be turned on and/or can be turned off. Accordingly, the response along the Th1 and Th2 signaling pathways for the creation of T Cytotoxic cells or antibodies can be turned on, or can be turned off (e.g., the Th1-Th2 switch can be controlled to direct more or less of either immune pathway being invoked). Similarly, the innate immune system and resultant inflammation can be turned on or can be turned off.
[0331] With the knowledge that one or more signaling pathways can be turned on/off, very important therapeutic treatments can thus occur. For example, a variety of surrogate endpoints can be monitored or examined for a variety of different diseases, including, for example, many cancers. For example, the antigen, “carcino-embryonic antigen” or “CEA” is a known surrogate endpoint marker for the amount of tumor or the amount of tumor burden present in a variety of different cancers. For example, it is known that the higher the CEA amount, the more tumors there are associated with ovarian cancer, breast cancer, colon cancer, rectal cancer, pancreatic cancer, lung cancer, etc. In this regard, the amount of carcino-embryonic antigen can be measured by, for example, drawing blood and testing for the presence of CEA by known techniques including, for example, ELISA and certain spectroscopy techniques. In this regard, once blood is drawn and a measurement is made to determine the amount of CEA, the extent of treatment required (e.g., the dose, duration and/or the amount) can be driven by monitoring the change in the amount of CEA measured. For example, if 15-45 ml of 10 ppm product is taken 2-3 times per day, monitoring of the amount of CEA could cause an increase in dosage, or a decrease in dosage, depending on the desired outcome.
[0332] Likewise, prostate cancer has a known surrogate endpoint of “prostate-specific antigen” or “PSA”. This surrogate endpoint can also be monitored by drawing blood and searching for the same by ELISA techniques.
[0333] Still further, various cancers, like melanoma (e.g., ocular, etc.) also express antigens for example “GP100” and/or “Melan-A”. These surrogate endpoints can also be determined by drawing blood from a patient and then measuring by similar ELISA or spectrographic techniques for the amount of antigen present. In all such cases, the presence of antigen can cause an increase/decrease in the amount of therapeutic treatment provided.
[0334] The following “Table A” sets forth a number of known “Tumor Markers” and associated cancers, as well as where biological samples are drawn to measure such markers.
TABLE-US-00002 TABLE A Common Tumor Markers Currently in Use Tumor Markers Cancers Usual sample AFP Liver, germ cell cancer Blood (Alpha-feto protein) of ovaries or testes B2M Multiple myeloma and Blood (Beta-2 microglobulin) lymphomas CA 15-3 Breast cancer and others, Blood (Cancer antigen 15-3) including lung, ovarian CA 19-9 Pancreatic, sometimes Blood (Cancer antigen 19-9) colorectal and bile ducts CA-125 Ovarian Blood (Cancer antigen 125) Calcitonin Thyroid medullary Blood carcinoma CEA Colorectal, lung, breast, Blood (Carcino-embryonic thyroid, pancreatic, liver, antigen) cervix, and bladder Chromogranin A Neuroendocrine tumors Blood (CgA) (carcinoid tumors, neuro- blastoma) Estrogen receptors Breast Tissue hCG (Human chorionic Testicular and tropho- Blood, urine gonadotropin) blastic disease Her-2/neu Breast Tissue Monoclonal Multiple myeloma and Blood, urine immunoglobulins Waldenstrom's macro- globulinemia Progesterone receptors Breast Tissue PSA (Prostate specific Prostate Blood antigen), total and free Thyroglobulin Thyroid Blood Other Tumor Markers Less Widely Used BTA Bladder Urine (Bladder tumor antigen) CA 72-4 Ovarian Blood (Cancer antigen 72-4) Des-gamma-carboxy Hepatocellular Blood prothrombin (DCP) carcinoma (HCC) EGFR (Her-1) Solid tumors, such as of Tissue the lung (non small cell), head and neck, colon, pancreas, or breast NSE Neuroblastoma, small cell Blood (Neuron-specific enolase) lung cancer NMP22 Bladder Urine Prostatic acid Metastatic prostate cancer, Blood phosphatase (PAP) myeloma, lung cancer Soluble Mesothelin- Mesothelioma Blood Related Peptides (SMRP)
[0335] Still further, various diseases of immune and inflammation dysfunction, like rheumatoid arthritis and Crohn's can be assessed using inflammatory markers such as C Reactive Protein (CRP) or erythrocyte sedimentation rate (ESR). These surrogate endpoints can also be determined by drawing blood from a patient and then measuring by visual ELISA or spectrographic techniques for the amount of marker present. In all such cases, the change in an inflammatory/immune marker can cause an increase/decrease in the amount of therapeutic treatment provided.
[0336] Still further, various antibody-based diseases, like hemolytic anemia or Rhesus disease, can be monitored by the concentration of specific antibodies present. These surrogate endpoints can also be determined by drawing blood from a patient and then measuring, by similar ELISA or spectrographic techniques, for the amount of antibody present. In all such cases, the presence of antibody can cause an increase/decrease in the amount of therapeutic treatment provided.
[0337] Inhibitors or modifiers of MIF and/or one or more of MIF's signaling pathway(s) may also be used in implantable devices such as stents. Accordingly, in a further aspect the present invention provides an implantable device, preferably a stent, comprising:
[0338] (i) a reservoir containing at least one compound of metallic-based compound comprising gold solutions or colloids and mixtures and alloys thereof; and
[0339] (ii) means to release or elute the inhibitor or modifier from the reservoir.
[0340] According to the invention therefore, there are a variety of indications that the nanocrystalline gold-based therapies of the present invention will have desirable efficacy against including various autoimmune diseases, tumors, or chronic or acute inflammatory conditions or diseases, disorders, syndromes, states, tendencies or predispositions, etc., selected from the group comprising:
[0341] rheumatic diseases (including but not limited to rheumatoid arthritis, osteoarthritis, psoriatic arthritis, Still's disease) spondyloarthropathies (including but not limited to ankylosing spondylitis, reactive arthritis, Reiter's syndrome), crystal arthropathies (including but not limited to gout, pseudogout, calcium pyrophosphate deposition disease), Lyme disease, polymyalgia rheumatica;
[0342] connective tissue diseases (including but not limited to systemic lupus erythematosus, systemic sclerosis, scleroderma, polymyositis, dermatomyositis, Sjogren's syndrome);
[0343] vasculitides (including but not limited to polyarteritis nodosa, Wegener's granulomatosis, Churg-Strauss syndrome);
[0344] inflammatory conditions or tendencies including consequences of trauma or ischemia; sarcoidosis;
[0345] vascular diseases including atherosclerotic vascular disease and infarction, atherosclerosis, and vascular occlusive disease (including but not limited to atherosclerosis, ischemic heart disease, myocardial infarction, stroke, peripheral vascular disease), and vascular stent restenosis;
[0346] ocular diseases including uveitis, corneal disease, iritis, iridocyclitis, and cataracts;
[0347] autoimmune diseases (including but not limited to diabetes mellitus, thyroiditis, myasthenia gravis, sclerosing cholangitis, primary biliary cirrhosis);
[0348] pulmonary diseases (including but not limited to diffuse interstitial lung diseases, pneumoconiosis, fibrosing alveolitis, asthma, bronchitis, bronchiectasis, chronic obstructive pulmonary disease, adult respiratory distress syndrome);
[0349] cancers whether primary or metastatic (including but not limited to prostate cancer, colon cancer, bladder cancer, kidney cancer, lymphoma, lung cancer, melanoma, multiple myeloma, breast cancer, stomach cancer, leukemia, cervical cancer and metastatic cancer);
[0350] renal diseases including glomerulonephritis, interstitial nephritis;
[0351] disorders of the hypothalamic-pituitary-adrenal axis;
[0352] nervous system disorders including multiple sclerosis, Alzheimer's disease, Parkinson's Disease, Huntington's disease;
[0353] diseases characterized by modified angiogenesis (e.g., diabetic retinopathy, rheumatoid arthritis, cancer) and endometriosis;
[0354] infectious diseases, including but not limited to bacterial, parasites or viral, including HIV, HBV, HCV, tuberculosis, malaria, and worms (including the current FDA designated neglected diseases of the developing world).
[0355] complications of infective disorders including endotoxic (septic) shock, exotoxic (septic) shock, infective (true septic) shock, complications of malaria (e.g., cerebral malaria and anemia), other complications of infection, and pelvic inflammatory disease;
[0356] transplant rejection, graft-versus-host disease;
[0357] allergic diseases including allergies, atopic diseases, allergic rhinitis;
[0358] bone diseases (e.g., osteoporosis, Paget's disease);
[0359] skin diseases including psoriasis, eczema, atopic dermatitis, UV(B)-induced dermal cell activation (e.g., sunburn, skin cancer);
[0360] diabetes mellitus and its complications;
[0361] pain, testicular dysfunctions and wound healing;
[0362] gastrointestinal diseases including inflammatory bowel disease (including but not limited to ulcerative colitis, Crohn's disease), peptic ulceration, gastritis, esophagitis, liver disease (including but not limited to cirrhosis and hepatitis).
[0363] In one embodiment, the disease or condition is selected from the group consisting of rheumatoid arthritis, osteo arthritis, systemic lupus erythematosus, ulcerative colitis, Crohn's disease, multiple sclerosis, psoriasis, eczema, uveitis, diabetes mellitus, glomerulonephritis, atherosclerotic vascular disease and infarction, asthma, chronic obstructive pulmonary disease, HIV, HBV, HCV, tuberculosis, malaria, worms, and cancer(s).
[0364] III. Pharmaceutical Compositions
[0365] Pharmaceutical compositions which include an effective amount of the gold nanocrystals to treat any of the medical conditions described in this application are also provided. In a preferred embodiment, the gold nanocrystals are administered in an orally delivered liquid, wherein the gold nanocrystals remain in the water of manufacture which may be concentrated or reconstituted, but preferable not dried to the point that the surfaces of the gold nanocrystals become completely dry or have their surfaces otherwise altered from their pristine state of manufacture.
[0366] Based on experiments, it appears that the present gold nanocrystals are a more potent form of gold than prior art gold-based materials, including both FDA-approved gold-based pharmaceutical products, and non-FDA-approved gold colloids, due to the substantially clean very active crystalline surfaces. Because of this, it is expected that significantly lower doses of the present nanocrystals can be used, than dose levels required by prior art compositions, including the oral gold product Auranofin.
[0367] For example, in the widely accepted collagen induced arthritis mouse model, a standard dose is 40 mg/kg/day of Auranofin, which is approximately 1 mg/mouse/day of Auranofin, and 0.30 mg gold/day of gold contained in Auranofin. This standard Auranofin dose level appears to give an equivalent response to that resulting from a dose of about 0.06 mg/day of the gold nanocrystals of the present invention (Example 25). Thus, in such experiment, the present nanocrystals were calculated to be 17 times more potent than was the Auranofin, and 5 times more potent than the gold species contained in the Auranofin.
[0368] The standard FDA-approved dose level for Auranofin in humans is 6 mg/day, or 0.9 mg/kg/day. The gold contained in that human dose levels of Auranofin is 1.74 mg, or 0.025 mg/kg. Given the relative potency of the novel gold nanocrystals compared to that of Auranofin, as demonstrated in the live animal model, an approximate human dose level for the novel gold nanocrystal can be calculated by dividing the human dose level for Auranofin by the relative potency factor of 17×, or by dividing the human dose level of the gold contained in the Auranofin by the relative potency factor of 5×. This results in an approximate human dose level for the novel gold nanocrystals of 0.35 mg/day, versus the 6 mg/day required for Auranofin, and 1.74 mg/day required for gold contained in Auranofin. 0.35 mg/day, for a 70 kg human being, is a dose of 0.005 mg/kg/day.
[0369] It is normal in developing dosing levels to establish a range of one order of magnitude or more surrounding an estimated mg/kg dose. In this case, if the approximate suggested base dose is 1/17 that of the base dose of Auranofin, or 0.348 mg/day, which is 0.005 mg/kg/day, this suggests that an effective dosing range for Auranofin-like efficacy with the novel nanocrystals can be achieved at dosing levels of 0.005 mg/kg/day, and even greater efficacy at levels in the range of 0.01 mg/kg/day or 0.25 mg/kg/day.
[0370] It is important to recognize that in pharmaceutical products the objective is to establish the minimum dose necessary to achieve efficacy, thus minimizing potential for toxicity or complications. A new orally administered product with significantly greater potency can achieve efficacy at dose levels below those of prior art products, and/or can achieve substantially greater efficacy at equivalent dose levels.
[0371] Moreover, it is observed in animal trials that toxicity levels of the novel nanocrystals are low, even at maximum dose levels, which means that even at higher dose levels there is less toxicity than with current products such as Auranofin.
[0372] It has also been observed in mice that a therapeutic effect is seen faster than with Auranofin, which has a typical onset of action of weeks, compared to days for the present nanocrystals (See Example 25). This is a major advantage in use, since it means patients enjoy relief sooner, and are much more likely to continue to comply with the regimen and thus continue to benefit from the product.
[0373] It has further been observed that the present gold nanocrystals have a better therapeutic index than Auranofin due to the lower dose required to achieve efficacy and the associated lower toxicity.
[0374] It is also important to recognize that to have real value as a pharmaceutical treatment, a product must be manufacturable under high pharmaceutical-grade manufacturing, sourcing, and quality control standards, as defined by the FDA as Good Manufacturing Practice (GMP). Conventional gold nanoparticles are made by a variety of methods, most of which involve chemical reduction processes. There appear to be no current chemical reduction or other conventional processes for production of gold nanoparticles which comply with GMP, and given the nature of these processes, it appears that GMP compliance, if possible, will be extremely challenging and will require substantial time, money, and inventive engineering to achieve. The process by which the present novel gold nanocrystals are produced is designed to be GMP compliant, establishing another major difference and advantage of the present gold nanocrystals.
[0375] While clinical trials are required to confirm the therapeutically efficacious dose, it is reasonable to conclude that doses ranging from 0.05 mgs or more (or 0.1, 0.5, 1.0, 2.0 mg or more) to 10 mg or more per dosage (once, twice or multiple times per day) are effective in a human to treat any of the conditions described herein. Given the low toxicity of these gold nanocrystals, for more problematic disorders it is appropriate to use at higher dose levels, including but not limited dosages of 10 mgs or more, such as 20 mg or more per dosage.
[0376] Any concentration of gold nanocrystals can be provided according to the invention. For example, concentrations of these gold nanocrystals can be a few parts per million (i.e., μg/ml or mg/l) up to a few hundred ppm, but are typically in the range of 2-200 ppm (i.e., 2 μg/ml-200 μg/ml) and more often in the range of 2-50 ppm (i.e., 2 μg/ml-50 μg/ml). A typical convenient concentration may be around 5-20 μg/ml, and more typically about 8-15 μg/ml.
[0377] Pharmaceutical compositions are provided that are appropriate for systemic or topical use, including oral, intravenous, subcutaneous, intra-arterial, buccal, inhalation, aerosol, propellant or other appropriate liquid, etc, as described further herein, including specific gels or creams discussed in Example 23.
[0378] Alternatively, suitable dosages of active ingredient may lie within the range of about 0.1 ng per kg of body weight to about 1 g per kg of body weight per dosage. The dosage is typically in the range of 1 μg to 1 g per kg of body weight per dosage, such as is in the range of 1 mg to 1 g per kg of body weight per dosage. In one embodiment, the dosage is in the range of 1 mg to 500 mg per kg of body weight per dosage. In another embodiment, the dosage is in the range of 1 mg to 250 mg per kg of body weight per dosage. In yet another preferred embodiment, the dosage is in the range of 1 mg to 100 mg per kg of body weight per dosage, such as up to 50 mg per kg of body weight per dosage. In yet another embodiment, the dosage is in the range of 1 μg to 1 mg per kg of body weight per dosage.
[0379] Suitable dosage amounts and dosing regimens can be determined by the attending physician or veterinarian and may depend on the desired level of inhibiting and/or modifying activity, the particular condition being treated, the severity of the condition, whether the dosage is preventative or therapeutic, as well as the general age, health and weight of the subject.
[0380] The gold nanocrystals contained in, for example, an aqueous medium, colloid, suspension, foam, gel, paste, liquid, cream or the like, may be administered in a single dose or a series of doses. While it is possible for the aqueous medium containing the metallic-based nanocrystals to be administered alone in, for example, colloid form, it may be acceptable to include the active ingredient mixture with other compositions and or therapies. Further, various pharmaceutical compositions can be added to the active ingredient(s)/suspension(s)/colloid(s).
[0381] Accordingly, typically, the inventive gold nanocrystal suspensions or colloids (e.g., comprising aqueous gold-based metal and/or mixtures of gold and other metal(s) and/or alloys of gold with other metal(s) and/or a combination therapy approach) are administered in conjunction with a second therapeutic agent. More typically, the second therapeutic agent comprises a glucocorticoid.
[0382] In a further aspect of the invention, there is provided a pharmaceutical composition comprising the inventive gold nanocrystal suspensions or colloids (e.g., comprising aqueous gold-based metal and/or mixtures of gold and other metal(s) and/or alloys of gold with other metal(s) and/or a combination therapy approach) together with a pharmaceutically acceptable carrier, diluent or excipient. The formulation of such compositions is well known to those skilled in the art. The composition may contain pharmaceutically acceptable additives such as carriers, diluents or excipients. These include, where appropriate, all conventional solvents, dispersion agents, fillers, solid earners, coating agents, antifungal and/or antibacterial agents, dermal penetration agents, ibuprofen, ketoprofen, surfactants, isotonic and absorption agents and the like. It will be understood that the compositions of the invention may also include other supplementary physiologically active agents. Still further, a large variety of dietary supplements and homeopathic carriers can also be utilized. Specifically, choices of such ingredients can be based in part on known functionality or use of these ingredients such that when combined with active ingredients of the invention, additive or synergistic affects can be achieved.
[0383] The carrier should be pharmaceutically acceptable in the sense of being compatible with the other ingredients in the inventive gold nanocrystal suspensions and not injurious (e.g., toxic at therapeutically active amounts) to the subject. Compositions include those suitable for oral, rectal, inhalational, nasal, transdermal, topical (including buccal and sublingual), vaginal or parenteral (including subcutaneous, intramuscular, intraspinal, intravenous and intradermal) administration. The compositions may conveniently be presented in unit dosage form and may be prepared by any methods well known in the art of pharmacy, homeopathy and/or dietary supplements. Such methods include the step of bringing into association the inventive metallic-based nanocrystals or suspensions with the carrier which constitutes one or more accessory ingredients. In general, the compositions are prepared by uniformly and intimately bringing into association one or more active ingredients in the solution/colloid under appropriate non-reactive conditions which minimize or eliminate, to the extent possible, negative or adverse reactions.
[0384] Depending on the disease or condition to be treated, it may or may not be desirable for the inventive gold nanocrystal suspensions or colloids to cross the blood/brain barrier.
[0385] Thus, the gold nanocrystal suspensions or colloids of the present invention may be manufactured to be of desirable size, desirable crystal plane(s) and/or desirable shapes or shape distributions, etc (as discussed elsewhere herein) to assist in crossing the blood/brain barrier.
[0386] Gold nanocrystal suspensions according to the present invention suitable for oral administration are presented typically as a stable solution, colloid or a partially stable suspension in water. However, such gold nanocrystals may also be included in a non-aqueous liquid, as discrete units such as liquid capsules, sachets or even tablets (e.g., drying-out suspensions or colloids to result in active ingredient gold-based nanocrystals so long as such processing does not adversely affect the functionality of the pristine gold nanocrystal surfaces) each containing a predetermined amount, of, for example, the gold nanocrystal active ingredient; as a powder or granules; as a solution, colloid or a suspension in an aqueous or as non-aqueous liquid; or as an oil-in-water liquid emulsion or a water-in-oil liquid emulsion. The gold nanocrystal active ingredient may also be combined into a bolus, electuary or paste.
[0387] A tablet made from the inventive gold nanocrystal suspensions or colloids (e.g., comprising aqueous gold-based nanocrystals and/or alloys of gold with other metal(s) and/or a combination therapy approach) and other materials or compounds may be made by, for example, first drying the suspension or colloid, collecting residual dried material and by compression or molding, forcing the powder into a suitable tablet or the like. For example, compressed tablets may be prepared by compressing in, a suitable machine, the active ingredient nanocrystals, for example, the metallic-based nanocrystals, in a free-flowing form such as a powder or granules, optionally mixed with a binder (e.g., inert diluent, preservative, disintegrant (e.g., sodium starch glycolate, cross-linked polyvinyl pyrrolidone, cross-linked sodium carboxymethyl cellulose)) surface-active or dispersing agent. Molded tablets may be made by, for example, molding or pressing in a suitable machine a mixture of the powdered compound moistened with an inert liquid diluent. The tablets may optionally be coated or scored and may be formulated so as to provide slow or controlled release of the active ingredient therein using, for example, hydroxypropylmethyl cellulose in varying proportions to provide the desired release profile. Tablets may optionally be provided with an enteric coating, to provide for release in parts of the gut other than the stomach.
[0388] Compositions suitable for topical administration in the mouth include lozenges comprising suspensions or colloids containing one or more active ingredient(s) gold nanocrystal in a flavored base, such as sucrose and acacia or tragacanth gum; pastilles comprising the gold nanocrystal active ingredient in an inert base such as a gelatin and a glycerin, or sucrose and acacia gum; and mouthwashes comprising the gold nanocrystal active ingredient in a suitable liquid carrier.
[0389] The inventive gold nanocrystal suspensions or colloids (e.g., comprising aqueous gold-based metal and/or mixtures of gold and other metal(s) and/or alloys of gold with other metal(s) and/or a combination therapy approach) may also be administered intranasally or via inhalation, for example by atomizer, aerosol or nebulizer means for causing one or more constituents in the solution or colloid (e.g., the gold nanocrystals) to be, for example, contained within a mist or spray.
[0390] Compositions suitable for topical administration to the skin may comprise the gold nanocrystals of the invention suspended in any suitable carrier or base and may be in the form of lotions, gel, creams, pastes, ointments and the like. Suitable carriers include mineral oil, propylene glycol, polyoxyethylene, polyoxypropylene, emulsifying wax, sorbitan monostearate, polysorbate 60, cetyl esters wax, cetearyl alcohol, 2-octyldodecanol, benzyl alcohol, carbopol and water.
[0391] Transdermal devices, such as patches, may also be used to administer the compounds of the invention.
[0392] Compositions for rectal administration may be presented as a suppository with a suitable carrier base comprising, for example, cocoa butter, gelatin, glycerin or polyethylene glycol.
[0393] Compositions suitable for vaginal administration may be presented as pessaries, tampons, creams, gels, pastes, foams or spray formulations containing in addition to the active ingredient such carriers as are known in the art to be appropriate.
[0394] Compositions suitable for parenteral administration include aqueous and non-aqueous isotonic sterile injection suspensions or colloids which may contain anti-oxidants, buffers, bactericides and solutes which render the composition isotonic with the blood of the intended recipient; and aqueous and non-aqueous sterile suspensions which may include suspending agents and thickening agents. The compositions may be presented in unit-dose or multi-dose sealed containers, for example, ampoules and vials, and may be stored in a freeze-dried (lyophilised) condition requiring only the addition of the sterile liquid carrier, for example water for injections, immediately prior to use. Extemporaneous injection solutions, colloids and suspensions may be prepared from sterile powders, granules and tablets of the kind previously described.
[0395] Preferred unit dosage compositions are those containing a daily dose or unit, daily sub-dose, as herein above described, or an appropriate fraction thereof, of the active ingredient.
[0396] It should be understood that in addition to the gold nanocrystal active ingredients particularly mentioned above, the compositions of this invention may include other agents conventional in the art having regard to the type of composition in question, for example, those suitable for oral administration may include such further agents as binders, sweeteners, thickeners, flavoring agents, disintegrating agents, coating agents, preservatives, lubricants, time delay agents and/or position release agents. Suitable sweeteners include sucrose, lactose, glucose, aspartame or saccharine. Suitable disintegrating agents include corn starch, methylcellulose, polyvinylpyrrolidone, xanthan gum, bentonite, alginic acid or agar. Suitable flavoring agents include peppermint oil, oil of wintergreen, cherry, orange or raspberry flavoring. Suitable coating agents include polymers or copolymers of acrylic acid and/or methacrylic acid and/or their esters, waxes, fatty alcohols, zein, shellac or gluten. Suitable preservatives include sodium benzoate, vitamin E, alpha-tocopherol, ascorbic acid, methyl paraben, propyl paraben or sodium bisulphite. Suitable lubricants include magnesium stearate, stearic acid, sodium oleate, sodium chloride or talc. Suitable time delay agents include glyceryl mono stearate or glyceryl distearate.
[0397] Further, by following the inventive electrochemical manufacturing processes of the invention, these gold-based metallic nanocrystals can be alloyed or combined with other metals in liquids such that gold “coatings” may occur on other metals (or other non-metal species such as SiO.sub.2, for example) or alternatively, gold-based nanocrystals may be coated by other metals. In such cases, gold-based composites or alloys may result within a colloid or suspension. Further, certain composites which include both gold and other metals can also be formed.
[0398] Still further, gold-based metallic nanocrystals suspensions or colloids of the present invention can be mixed or combined with other metallic-based solutions or colloids to form novel solution or colloid mixtures (e.g., in this instance, distinct metal species can still be discerned).
[0399] IV. Method of Manufacturing Gold Nanocrystals
[0400] A novel process is provided to produce these unique gold nanocrystals. The process involves the creation of the gold nanocrystals in water. In a preferred embodiment, the water contains an added “process enhancer” which does not significantly bind to the formed nanocrystals, but rather facilitates nucleation/crystal growth during the electrochemical-stimulated growth process. The process enhancer serves important roles in the process including providing charged ions in the electrochemical solution to permit the crystals to be grown. These novel electrochemical processes can occur in either a batch, semi-continuous or continuous process. These processes result in controlled gold nanocrystalline concentrations, controlled nanocrystal sizes and controlled nanocrystal size ranges; as well as controlled nanocrystal shapes and controlled nanocrystal shape distributions. Novel manufacturing assemblies are provided to produce these gold nanocrystals.
[0401] In one preferred embodiment, the gold-based nanocrystal suspensions or colloids are made or grown by electrochemical techniques in either a batch, semi-continuous or continuous process, wherein the amount, average particle size, crystal plane(s) and/or particle shape(s) and/or particle shape distributions are controlled and/or optimized to achieve high biological activity and low cellular/biologic toxicity (e.g., a high therapeutic index). Desirable average crystal sizes include a variety of different ranges, but the most desirable ranges include average crystal sizes that are predominantly less than 100 nm and more typically, for many uses, less than 50 nm and even more typically for a variety of, for example, oral uses, less than 30 nm, and in many of the preferred embodiments disclosed herein, the mode for the nanocrystal size distribution is less than 21 nm and within an even more preferable range of 8-18 nm, as measured by drying such solutions and constructing particle size histograms from TEM measurements (as described in more detail herein). Further, the particles desirably contain crystal planes, such desirable crystal planes including crystals having {111}, {110} and/or {100} facets, which can result in desirable crystal shapes and desirable crystal shape distributions and better performance than gold spherical or randomly-shaped particles.
[0402] Further, by following the inventive electrochemical manufacturing processes of the invention, these gold-based metallic nanocrystals can be alloyed or combined with other metals in liquids such that gold “coatings” may occur on other metals (or other non-metal species such as SiO.sub.2, for example) or alternatively, gold-based nanocrystals may be coated by other metals. In such cases, gold-based composites or alloys may result within a colloid or suspension. Further, certain composites which include both gold and other metals can also be formed.
[0403] Still further, gold-based metallic nanocrystals suspensions or colloids of the present invention can be mixed or combined with other metallic-based solutions or colloids to form novel solution or colloid mixtures (e.g., in this instance, distinct metal species can still be discerned).
[0404] Methods for making novel metallic-based nanocrystal suspensions or colloids according to the invention relate generally to novel methods and novel devices for the continuous, semi-continuous and batch manufacture of a variety of constituents in a liquid including micron-sized particles, nanocrystals, ionic species and aqueous-based compositions of the same, including, nanocrystal/liquid(s), solution(s), colloid(s) or suspension(s). The constituents and nanocrystals produced can comprise a variety of possible compositions, concentrations, sizes, crystal planes (e.g., spatially extended low index crystal planes) and/or shapes, which together can cause the inventive compositions to exhibit a variety of novel and interesting physical, catalytic, biocatalytic and/or biophysical properties. The liquid(s) used and created/modified during the process can play an important role in the manufacturing of, and/or the functioning of the constituents (e.g., nanocrystals) independently or synergistically with the liquids which contain them. The particles (e.g., nanocrystals) are caused to be present (e.g., created and/or the liquid is predisposed to their presence (e.g., conditioned)) in at least one liquid (e.g., water) by, for example, typically utilizing at least one adjustable plasma (e.g., created by at least one AC and/or DC power source), which adjustable plasma communicates with at least a portion of a surface of the liquid. However, effective constituent (e.g., nanocrystals) suspensions or colloids can be achieved without the use of such plasmas as well.
[0405] Metal-based electrodes of various composition(s) and/or unique configurations or arrangements are preferred for use in the formation of the adjustable plasma(s), but non-metallic-based electrodes can also be utilized for at least a portion of the process. Utilization of at least one subsequent and/or substantially simultaneous adjustable electrochemical processing technique is also preferred. Metal-based electrodes of various composition(s) and/or unique configurations are preferred for use in the electrochemical processing technique(s). Electric fields, magnetic fields, electromagnetic fields, electrochemistry, pH, zeta potential, chemical/crystal constituents present, etc., are just some of the variables that can be positively affected by the adjustable plasma(s) and/or adjustable electrochemical processing technique(s) of the invention. Multiple adjustable plasmas and/or adjustable electrochemical techniques are preferred in many embodiments of the invention to achieve many of the processing advantages of the present invention, as well as many of the novel nanocrystals and nanocrystal compositions which result from practicing the teachings of the preferred embodiments to make an almost limitless set of inventive aqueous solutions, suspensions and/or colloids.
[0406] In the continuous process embodiments of the invention, at least one liquid, for example water, flows into, through and out of at least one trough member and such liquid is processed, conditioned, modified and/or effected by said at least one adjustable plasma and/or said at least one adjustable electrochemical technique. The results of the continuous processing include new constituents in the liquid, micron-sized particles, ionic constituents, nanocrystals (e.g., metallic-based nanocrystals) of novel and/or controllable size, hydrodynamic radius, concentration, crystal sizes and crystal size ranges, crystal planes, spatially extended low index crystal planes, crystal shapes and distributions of crystal shapes and, composition, zeta potential, pH and/or properties, such nanocrystal/liquid mixture being produced in an efficient and economical manner.
[0407] In a preferred embodiment, the process involves the nucleation and growth of the gold nanocrystals in water which contains a “process enhancer” or “processing enhancer” (typically an inorganic material) which does not significantly bind to the formed nanocrystals, but rather facilitates nucleation/growth during electrochemical-stimulated growth process. The process enhancer serves important roles in the process including providing charged ions in the electrochemical solution to permit the crystals to be grown. The process enhancer is critically a compound(s) which remains in solution, and/or does not form a coating (e.g., an organic coating), and/or does not adversely affect the formed nanocrystals or the formed suspension(s), and/or is destroyed, evaporated, or is otherwise lost during the electrochemical process. A preferred process enhancer is sodium bicarbonate. Examples of other process enhancers are sodium carbonate, potassium bicarbonate, potassium carbonate, trisodium phosphate, disodium phosphate, monosodium phosphate, potassium phosphates or other salts of carbonic acid or the like. Further process enhancers may be salts, including sodium or potassium, of bisulfite or sulfite. Still other process enhancers to make gold nanocrystals for medical applications under certain conditions may be other salts, including sodium or potassium, or any material that assists in the electrochemical growth processes described herein; and any material is not substantially incorporated into or onto the surface of the gold nanocrystals; and does not impart toxicity to the nanocrystals or to the suspension containing the nanocrystals.
[0408] Desirable concentration ranges for the processing enhancer include typically 0.01-20 grams/gallon (0.0026-2.1730 mg/ml), more typically, 0.1-7.5 grams/gallon (0.0264-1.9813 mg/ml) and most typically, 0.5-2.0 grams/gallon (0.13210-0.5283 mg/ml).
[0409] For example, certain processing enhancers may dissociate into positive ions (cations) and negative ions (anions). The anions and/or cations, depending on a variety of factors including liquid composition, concentration of ions, applied fields, frequency of applied fields, waveform of the applied filed, temperature, pH, zeta potential, etc., will navigate or move toward oppositely charged electrodes. When said ions are located at or near such electrodes, the ions may take part in one or more reactions with the electrode(s) and/or other constituent(s) located at or near such electrode(s). Sometimes ions may react with one or more materials in the electrode (e.g., when NaCl is used as a processing enhancer, various metal chloride (MCl, MCl.sub.2, etc.) may form). Such reactions may be desirable in some cases or undesirable in others. Further, sometimes ions present in a solution between electrodes may not react to form a product such as MCl, MCl.sub.2, etc., but rather may influence material in the electrode (or near the electrode) to form metallic nano-crystals that are “grown” from material provided by the electrode. For example, certain metal ions may enter the liquid 3 from the electrode 5 and be caused to come together (e.g., nucleate) to form constituents (e.g., ions, nanocrystals, etc.) within the liquid 3.
[0410] Further, it is important to select a process enhancer that will not impart toxicity to the gold nanocrystal or the liquid that the crystal is in to maximize pharmaceutical acceptability. For example, for certain applications, chloride ion may be undesired if it creates gold chloride salts which may have toxicity.
[0411] Further, depending upon the specific formed products, drying, concentrating and/or freeze drying can also be utilized to remove at least a portion of, or substantially all of, the suspending liquid, resulting in, for example, partially or substantially completely dehydrated nanocrystals. If solutions, suspensions or colloids are completely dehydrated, the metal-based species should be capable of being rehydrated by the addition of liquid (e.g., of similar or different composition than that which was removed). However, not all compositions/colloids of the present invention can be completely dehydrated without adversely affecting performance of the composition/colloid. For example, many nanocrystals formed in a liquid tend to clump or stick together (or adhere to surfaces) when dried. If such clumping is not reversible during a subsequent rehydration step, dehydration should be avoided.
[0412] In general, it is possible to concentrate, several folds, certain solutions, suspensions or colloids of gold made according to the invention, without destabilizing the composition. However, complete evaporation is difficult to achieve due to, for example, agglomeration effects. In many of the embodiments disclosed herein, such agglomeration effects seem to begin at an approximate volume of 30% of the initial or starting reference volume being removed from the suspension or colloid. Additionally, one can evaporate off a certain volume of liquid and subsequently reconstitute or add-back the amount of liquid evaporated to achieve a very similar product, as characterized by, for example, FAAS, DLS, and UV-Vis techniques. For Example, two 500 ml suspensions of nanocrystalline colloidal gold, made by techniques similar to those to manufacture GB-139 (discussed in detail in the Examples section herein) were each placed into a glass beaker and heated on a hot plate until boiling. The suspensions were evaporated to 300 mL and 200 mL, respectively, and later reconstituted with that amount of liquid which was removed (i.e., with water purified by deionization and reverse osmosis (“DI/RO”) water in 200 mL and 300 mL quantities, respectively) and subsequently characterized. Additionally, in another instance, two GB-139 suspension were again evaporated to 300 mL and 200 mL and then characterized without rehydration. It was found that these dehydration processes had little to no detrimental effects on the nanocrystal sizes or nanocrystal shapes (i.e., the nanocrystal size range and nanocrystal shape distributions did not change dramatically when the GB-139 colloid was dehydrated; or dehydrated and rehydrated to its initial gold concentration or ppm level).
[0413] One important aspect of the invention involves the creation of at least one adjustable plasma, which adjustable plasma is located between at least one electrode positioned adjacent to (e.g., above) at least a portion of the surface of a liquid (e.g., water) and at least a portion of the surface of the liquid itself. The liquid is placed into electrical communication with at least one second electrode (or a plurality of second electrodes) causing the surface of the liquid to function as an electrode, thus taking part in the formation of the adjustable plasma. This configuration has certain characteristics similar to a dielectric barrier discharge configuration, except that the surface of the liquid is an active electrode participant in this configuration.
[0414] Each adjustable plasma utilized can be located between the at least one electrode located above a surface of the liquid and a surface of the liquid due to at least one electrically conductive electrode being located somewhere within (e.g., at least partially within) the liquid. At least one power source (in a preferred embodiment, at least one source of volts and amps such as a transformer or power source) is connected electrically between the at least one electrode located above the surface of the liquid and the at least one electrode contacting the surface of the liquid (e.g., located at least partially, or substantially completely, within the liquid). The electrode(s) may be of any suitable composition and suitable physical configuration (e.g., size and shape) which results in the creation of a desirable plasma between the electrode(s) located above the surface of the liquid and at least a portion of the surface of the liquid itself.
[0415] The applied power (e.g., voltage and amperage) between the electrode(s) (e.g., including the surface of the liquid functioning as at least one electrode for forming the plasma) can be generated by any suitable source (e.g., voltage from a transformer) including both AC and DC sources and variants and combinations thereof. Generally, the electrode or electrode combination located within (e.g., at least partially below the surface of the liquid) takes part in the creation of a plasma by providing voltage and current to the liquid or solution. However, the adjustable plasma is actually located between at least a portion of the electrode(s) located above the surface of the liquid (e.g., at a tip or point thereof) and one or more portions or areas of the liquid surface itself. In this regard, the adjustable plasma can be created between the aforementioned electrodes (i.e., those located above at least a portion of the surface of the liquid and a portion of the liquid surface itself) when a breakdown voltage of the gas or vapor around and/or between the electrode(s) and the surface of the liquid is achieved or maintained.
[0416] In one embodiment of the invention, the liquid comprises water (or water containing certain processing enhancer(s)), and the gas between the surface of the water and the electrode(s) above the surface of the water (i.e., that gas or atmosphere that takes part in the formation of the adjustable plasma) comprises air. The air can be controlled to contain various different water content(s) or a desired humidity which can result in different compositions, concentrations, crystal size distributions and/or crystal shape distributions of constituents (e.g., nanocrystals) being produced according to the present invention (e.g., different amounts of certain constituents in the adjustable plasma and/or in the solution or suspension can be a function of the water content in the air located above the surface of the liquid) as well as different processing times required to obtain certain concentrations of various constituents in the liquid, etc. Specific aspects of the adjustable plasma 4 are discussed in greater detail in Examples 5-7.
[0417] The breakdown electric field at standard pressures and temperatures for dry air is about 3MV/m or about 30 kV/cm. Thus, when the local electric field around, for example, a metallic point exceeds about 30 kV/cm, a plasma can be generated in dry air. Equation (1) gives the empirical relationship between the breakdown electric field “E.sub.c” and the distance “d” (in meters) between two electrodes:
Of course, the breakdown electric field “E.sub.c” will vary as a function of the properties and composition of the gas or vapor located between electrodes. In this regard, in one preferred embodiment where water (or water containing a processing enhancer) is the liquid, significant amounts of water vapor can be inherently present in the air between the “electrodes” (i.e., between the at least one electrode located above the surface of the water and the water surface itself which is functioning as one electrode for plasma formation) and such water vapor should have an effect on at least the breakdown electric field required to create a plasma therebetween. Further, a higher concentration of water vapor can be caused to be present locally in and around the created plasma due to the interaction of the adjustable plasma with the surface of the water. The amount of “humidity” present in and around the created plasma can be controlled or adjusted by a variety of techniques discussed in greater detail later herein. Likewise, certain components present in any liquid can form at least a portion of the constituents forming the adjustable plasma located between the surface of the liquid and the electrode(s) located adjacent (e.g., along) the surface of the liquid. The constituents in the adjustable plasma, as well as the physical properties of the plasma per se, can have a dramatic influence on the liquid, as well as on certain of the processing techniques (discussed in greater detail later herein).
[0418] The electric field strengths created at and near the electrodes are typically at a maximum at a surface of an electrode and typically decrease with increasing distance therefrom. In cases involving the creation of an adjustable plasma between a surface of the liquid and the at least one electrode(s) located adjacent to (e.g., above) the liquid, a portion of the volume of gas between the electrode(s) located above a surface of a liquid and at least a portion of the liquid surface itself can contain a sufficient breakdown electric field to create the adjustable plasma. These created electric fields can influence, for example, behavior of the adjustable plasma, behavior of the liquid (e.g., influence the crystal state of the liquid) behavior of constituents in the liquid, etc.
[0419] In this regard,
[0420] The adjustable plasma region 4, created in the embodiment shown in
[0421] The composition of the electrode(s) 1 involved in the creation of the adjustable plasma(s) 4 of
[0422] Further, depending on, for example, electric, magnetic and/or electromagnetic field strength in and around the liquid 3 and the volume of liquid 3 exposed to such fields (discussed in greater detail elsewhere herein), the physical and chemical construction of the electrode(s) 1 and 5, atmosphere (naturally occurring or supplied), liquid composition, greater or lesser amounts of electrode(s) materials(s) (e.g., metal(s) or derivatives of metals) may be found in the liquid 3. In certain situations, the material(s) (e.g., metal(s) or metal(s) composite(s)) or constituents (e.g., Lewis acids, Bronsted-Lowry acids, etc.) found in the liquid 3 (permanently or transiently), or in the plasma 4, may have very desirable effects, in which case relatively large amounts of such materials will be desirable; whereas in other cases, certain materials found in the liquid 3 (e.g., by-products) may have undesirable effects, and thus minimal amounts of such materials may be desired in the liquid-based final product. Accordingly, electrode composition can play an important role in the materials that are formed according to the embodiments disclosed herein. The interplay between these components of the invention are discussed in greater detail later herein.
[0423] Still further, the electrode(s) 1 and 5 may be of similar chemical composition (e.g., have the same chemical element as their primary constituent) and/or mechanical configuration or completely different compositions (e.g., have different chemical elements as their primary constituent) in order to achieve various compositions and/or structures of liquids and/or specific effects discussed later herein.
[0424] The distance “y” between the electrode(s) 1 and 5; or 1 and 1 (shown later herein) or 5 and 5 (shown later herein) is one important aspect of the invention. In general, when working with power sources capable of generating a plasma under the operating condition, the location of the smallest distance “y” between the closest portions of the electrode(s) used in the present invention should be greater than the distance “x” in order to prevent an undesirable arc or formation of an unwanted corona or plasma occurring between the electrode (e.g., the electrode(s) 1 and the electrode(s) 5) (unless some type of electrical insulation is provided therebetween). Features of the invention relating to electrode design, electrode location and electrode interactions between a variety of electrodes are discussed in greater detail later herein.
[0425] The power applied through the power source 10 may be any suitable power which creates a desirable adjustable plasma 4 under all of the process conditions of the present invention. In one preferred mode of the invention, an alternating current from a step-up transformer is utilized. Preferred transformer(s) 60 (see e.g.,
[0426] The transformer 60 is rated for its secondary open circuit voltage and secondary short circuit current. Open circuit voltage (OCV) appears at the output terminals of the transformer 60 only when no electrical connection is present. Likewise, short circuit current is only drawn from the output terminals if a short is placed across those terminals (in which case the output voltage equals zero). However, when a load is connected across these same terminals, the output voltage of the transformer 60 should fall somewhere between zero and the rated OCV. In fact, if the transformer 60 is loaded properly, that voltage will be about half the rated OCV.
[0427] The transformer 60 is known as a Balanced Mid-Point Referenced Design (e.g., also formerly known as balanced midpoint grounded). This is most commonly found in mid to higher voltage rated transformers and most 60 mA transformers. This is the only type transformer acceptable in a “mid-point return wired” system. The “balanced” transformer 60 has one primary coil 601 with two secondary coils 603, one on each side of the primary coil 601 (as shown generally in the schematic view in
[0428] In another preferred embodiment, a rectified AC source creates a positively charged electrode 1 and a negatively charged surface 2 of the liquid 3. In another preferred embodiment, a rectified AC source creates a negatively charged electrode 1 and a positively charged surface 2 of the liquid 3. Further, other power sources such as RF power sources and/or microwave power sources can also be used with the present invention. In general, the combination of electrode(s) components 1 and 5, physical size and shape of the electrode(s) 1 and 5, electrode manufacturing process, mass of electrodes 1 and/or 5, the distance “x” between the tip 9 of electrode 1 above the surface 2 of the liquid 3, the composition of the gas between the electrode tip 9 and the surface 2, the flow rate (if any) and/or flow direction “F” of the liquid 3, the amount of liquid 3 provided, type of power source 10, frequency and/or waveform of the power output of the power source 10, all contribute to the design, and thus power requirements (e.g., breakdown electric field) required to obtain a controlled or adjustable plasma 4 between the surface 2 of the liquid 3 and the electrode tip 9.
[0429] In further reference to the configurations shown in
[0430]
[0431] Preferred techniques for automatically raising and/or lowering the electrodes 1, 5 are discussed later herein. The power source 10 can be connected in any convenient electrical manner to the electrodes 1 and 5. For example, wires 11a and 11b can be located within at least a portion of the electrode holders 6a, 6b (and/or electrical insulating portions 7a, 7b) with a primary goal being achieving electrical connections between the portions 11a, 11b and thus the electrodes 1, 5.
[0432]
[0433]
[0434] Likewise, a set of manually controllable electrode configurations, corresponding generally to
[0435]
[0436] Moreover, it should be understood that in alternative preferred embodiments of the invention, well defined sharp points are not always required for the tip 9. In this regard, the electrode 1 shown in
[0437]
[0438]
[0439]
[0440]
[0441] Likewise,
[0442]
[0443] Likewise,
[0444]
[0445]
[0446] The electrode configurations shown generally in
[0447]
[0448] Likewise, several additional alternative cross-sectional embodiments for the liquid-containing trough member 30 are shown in
[0449] Further, strong electric and magnetic field concentrations will also affect the interaction of the plasma 4 with the liquid 3 as well as affect the interaction of the electrode 5 with the liquid 3. Some important aspects of these important interactions are discussed in greater detail elsewhere herein. Further, a trough member 30 may comprise more than one cross-sectional shape along its entire longitudinal length. The incorporation of multiple cross-sectional shapes along the longitudinal length of a trough member 30 can result in, for example, varying the field or concentration or reaction effects (e.g., crystal growth/nucleation effects) being produced by the inventive embodiments disclosed herein (discussed in greater detail elsewhere herein). Further, a trough member 30 may not be linear or “I-shaped”, but rather may be “Y-shaped” or “Ψ-shaped”, with each portion of the “Y” (or “Ψ”) having a different (or similar) cross-sectional shape and/or set of dimensions and/or set of reaction conditions occurring therein.
[0450] Also, the initial temperature of the liquid 3 input into the trough member 30 can also affect a variety of properties of products produced according to the disclosure herein. For example, different temperatures of the liquid 3 can affect nanocrystal size(s) and nanocrystal shape(s), concentration or amounts of various formed constituents (e.g., transient, semi-permanent or permanent constituents), pH, zeta potential, etc. Likewise, temperature controls along at least a portion of, or substantially all of, the trough member 30 can have desirable effects. For example, by providing localized cooling, resultant properties of products formed (e.g., nanocrystal size(s) and/or nanocrystal shape(s)) can be controlled. Preferable liquid 3 temperatures during the processing thereof are between freezing and boiling points, more typically, between room temperature and boiling points, and even more typically, between about 40-98 degrees C., and more typically, between about 50-98 degrees C. Such temperature can be controlled by, for example, conventional means for cooling located at or near various portions of the processing apparatus.
[0451] Further, certain processing enhancers may also be added to or mixed with the liquid(s) 3. The processing enhancers include both solids and liquids (and gases in some cases). The processing enhancer(s) may provide certain processing advantages and/or desirable final product characteristics. Some portion of the processing enhancer(s) may function, influence as or become part of, for example, desirable seed crystals (or promote desirable seed crystals, or be involved in the creation of a nucleation site) and/or crystal plane growth promoters/preventers in the electrochemical growth processes of the invention; or may simply function as a current or power regulator in the electrochemical processes of the invention. Such processing enhancers may also desirably affect current and/or voltage conditions between electrodes 1/5 and/or 5/5.
[0452] A preferred processing enhancer is sodium bicarbonate. Examples of other process enhancers are sodium carbonate, potassium bicarbonate, potassium carbonate, trisodium phosphate, disodium phosphate, monosodium phosphate, potassium phosphates or other salts of carbonic acid or the like. Further process enhancers may be salts, including sodium or potassium, of bisulfite or sulfite. Still other process enhancers to make gold nanocrystals for medical applications under certain conditions may be other salts, including sodium or potassium, or any material that assists in the electrochemical growth processes described herein; and any material is not substantially incorporated into or onto the surface of the gold nanocrystals; and does not impart toxicity to the nanocrystals or to the suspension containing the nanocrystals. Processing enhancers may assist in 10 one or more of the electrochemical reactions disclosed herein; and/or may assist in achieving one or more desirable properties in products formed according to the teachings herein.
[0453] For example, certain processing enhancers may dissociate into positive ions (cations) and negative ions (anions). The anions and/or cations, depending on a variety of factors including liquid composition, concentration of ions, applied fields, frequency of applied fields, waveform of the applied filed, temperature, pH, zeta potential, etc., will navigate or move toward oppositely charged electrodes. When said ions are located at or near such electrodes, the ions may take part in one or more reactions with the electrode(s) and/or other constituent(s) located at or near such electrode(s). Sometimes ions may react with one or more materials in the electrode (e.g., when NaCl is used as a processing enhancer, various metal chloride (MCl, MCl.sub.2, etc.) may form). Such reactions may be desirable in some cases or undesirable in others. Further, sometimes ions present in a solution between electrodes may not react to form a product such as MCl, MCl.sub.2, etc., but rather may influence material in the electrode (or near the electrode) to form metallic nano-crystals that are “grown” from material provided by the electrode. For example, certain metal ions may enter the liquid 3 from the electrode 5 and be caused to come together (e.g., nucleate) to form constituents (e.g., ions, nanocrystals, etc.) within the liquid 3.
[0454] In the case of gold, a variety of extended surface planes from which crystal growth can occur are available, so long as impurities (such as, for example organic impurities) do not inhibit or prevent such growth. While gold is known to have a face centered cubic (fcc) structure, gold nanocrystals which are grown according to the methods of the present invention, are not single crystals and are typically twinned to result in a variety of desirable and highly reactive nanocrystalline shapes or shape distributions. For example, single crystal surfaces {111}, {100} and {110} are among the most frequently studied and well understood surfaces. The presence of certain species such as ions (e.g., added to or being donated by electrode 5) in an electrochemical crystal nucleation/growth process can influence (e.g., nucleate and/or promote growth of specifically-shaped nanocrystals or nanocrystal shape distributions) the presence or absence of one or more of such extended surfaces. A certain ion (e.g., anion) under certain field conditions may assist in the presence of more {111} extended surfaces or planes relative to other crystal surfaces which can result in the presence of certain nanocrystalline shapes relative to other shapes (e.g., more decahedron shapes relative to other shapes such as tetrahedrons, icosahedrons, octahedrons; or the combination(s) of certain crystalline shapes relative to other crystalline shapes, etc.). By controlling the presence or absence (e.g., relative amounts) of such faces, crystal shapes (e.g., hexagonal plates, octahedrons, tetrahedrons and pentagonal bipyramids (i.e., decahedrons)) and/or crystal sizes or extended crystal planes which contain such faces, nanocrystal shapes, can thus be relatively controlled. Control of the size and shape of nanocrystals (as well as the surface properties of nanocrystals) can control their function(s) in a variety of systems, including biological systems.
[0455] Specifically, the presence of certain nanocrystalline shapes (or shape distributions) containing specific spatially extended low index crystal planes can cause different reactions (e.g., different biocatalytic and/or biophysical reactions and/or cause different biological signaling pathways to be active/inactive relative to the absence of such shaped nanoparticles) and/or different reactions selectively to occur under substantially identical conditions. One crystalline shape of a gold nanoparticle (e.g., a pentagonal by-pyramidal structure, or decahedron, or tetrahedron containing {111} planes) can result in one set of reactions to occur (e.g., binding to a particular protein or homologue and/or affecting a particular biological signaling pathway of a protein or a cytokine) whereas a different crystal shape (e.g., a octahedron containing the same or different crystal planes such as {111} or {100}) can result in a different reaction endpoint (i.e., a different biocatalytic or signaling pathway effect). More dramatically, the lack of any extended crystal growth plane results in a spherical-shaped nanoparticle (e.g., such as those made by classical homogenous chemical reduction processes) significantly affects the performance of the nanoparticle (e.g., relative to an extended plane nanocrystal). Such differences in performance may be due to differing surface plasmon resonances and/or intensity of such resonances. Thus, by controlling amount (e.g., concentration), nanocrystal sizes, the presence or absence of certain extended growth crystal planes, and/or nanocrystalline shapes or shape distribution(s), certain reactions (e.g., biological reactions and/or biological signaling pathways) can be desirably influenced and/or controlled. Such control can result in the prevention and/or treatment of a variety of different diseases or indications that are a function of certain biologic reactions and/or signaling pathways (discussed later herein).
[0456] Further, certain processing enhancers may also include materials that may function as charge carriers, but may themselves not be ions. Specifically, metallic-based particles, either introduced or formed in situ (e.g., heterogeneous or homogenous nucleation/growth) by the electrochemical processing techniques disclosed herein, can also function as charge carriers, crystal nucleators and/or growth promoters, which may result in the formation of a variety of different crystalline shapes (e.g., hexagonal plates, octahedrons, tetrahedrons, pentagonal bi-pyramids (decahedrons), etc.). Once again, the presence of particular particle crystal sizes, extended crystal planes and/or shapes or shape distributions of such crystals, can desirably influence certain reactions (e.g., binding to a particular protein or protein homologue and/or affecting a particular biological signaling pathway such as an inflammatory pathway or a proteasomal pathway) to occur. Further, since the processing enhancers of the present invention do not contemplate those traditional organic-based molecules used in traditional reduction chemistry techniques, the lack of such chemical reductant (or added surfactant) means that the surfaces of the grown nanocrystals on the invention are very “clean” relative to nanoparticles that are formed by traditional reduction chemistry approaches. It should be understood that when the term “clean” is used with regard to nanocrystal surfaces or when the phrase “substantially free from organic impurities or films” (or a similar phrase) is used, what is meant is that the formed nanocrystals do not have chemical constituents adhered or attached to their surfaces which (1) alter the functioning of the nanocrystal and/or (2) form a layer, surface or film which covers a significant portion (e.g., at least 25% of the crystal, or more typically, at least 50% of the crystal). In preferred embodiments, the nanocrystal surfaces are completely free of any organic contaminants which materially change their functionality. It should be further understood that incidental components that are caused to adhere to nanocrystals of the invention and do not adversely or materially affect the functioning of the inventive nanocrystals, should still be considered to be within the metes and bounds of the invention. One example of a nanocrystal surface that is completely free from organic impurities or films is shown in Example 5 herein.
[0457] The lack of added chemicals (e.g., organics) permits the growth of the gold atoms into the extended crystal planes resulting in the novel crystalline shape distributions and also affects the performance of the nanocrystals in vivo (e.g., affects the protein corona formed around the nanoparticles/nanocrystals in, for example, serum). For example, but without wishing to be bound by any particular theory or explanation, protein corona formation can control location of a nanoparticle/nanocrystal in vivo, as well as control protein folding of proteins at or near the nanoparticle/nanocrystal surfaces. Such differences in performance may be due to such factors including, but not limited to, surface charge, surface plasmon resonance, epitaxial effects, surface double layers, zones of influence, and others.
[0458] Still further, once a seed crystal occurs in the process and/or a set of extended crystal planes begins to grow (e.g., homogenous nucleation) or a seed crystal is separately provided (e.g., heterogenous nucleation) the amount of time that a formed particle (e.g., a metal atom) is permitted to dwell at or near one or more electrodes in an electrochemical process can result in the size of such nanocrystals increasing as a function of time (e.g., metal atoms can assemble into metal nanocrystals and, if unimpeded by certain organic constituents in the liquid, they can grow into a variety of shapes and sizes). The amount of time that crystal nucleation/growth conditions are present can control the shape(s) and sizes(s) of grown nanocrystals. Accordingly, dwell time at/around electrodes, liquid flow rate(s), trough cross-sectional shape(s), etc, all contribute to nanocrystal growth conditions, as discussed elsewhere herein.
[0459] In a preferred embodiment the percent of pentagonal bipyramids is at least about 5%, or is in a range of about 5%-35%, and more typically at least about 10%, or is in a range of about 10%-35%, and even more typically, at least about 15%, or is in a range of about 15%-35%, and still more typically, at least about 25%, and in some cases at least about 30%.
[0460] In another preferred embodiment the percent of tetrahedrons is at least 5%, or is in a range of about 5%-35%, and more typically at least about 10%, or is in a range of about 10%-35%, and even more typically, at least about 15%, or is in a range of about 15%-35%, and still more typically, at least about 25%, and in some cases at least about 30%.
[0461] Still further, the combination of pentagonal bipyramids and tetrahedrons is at least about 15%, or is in a range of about 15%-50%, and more typically at least about 20%, or is in a range of about 20%-50%, and even more typically, at least about 30%, or is in a range of about 30%-50%, and still more typically, at least about 35%, and in some cases at least about 45%.
[0462] Still further, the combination of pentagonal bipyramids, tetrahedrons, octahedrons and hexagonal is at least about 50%, or is in a range of about 50%-85%, and more typically at least about 60%, or is in a range of about 60%-85%, and even more typically, at least about 70%, or is in a range of about 70%-85%, and still more typically, at least about 70%, and in some cases at least about 80%.
[0463] In many of the preferred embodiments herein, one or more AC sources are utilized. The rate of change from “+” polarity on one electrode to “−” polarity on the same electrode is known as Hertz, Hz, frequency, or cycles per second. In the United States, the standard output frequency is 60 Hz, while in Europe it is predominantly 50 Hz. As shown in the Examples herein, the frequency can also influence size and/or shape of nanocrystals formed according to the electrochemical techniques disclosed herein. Preferable frequencies are 5-1000 Hz, more typically, 20-500 Hz, even more typically, 40-200 Hz, and even more typically, 50-100 Hz. For example, and without wishing to be bound by any particular theory or explanation, nucleated or growing crystals can first have attractive forces exerted on them (or on crystal growth constituents, such as ions or atoms, taking part in forming the crystal(s)) due to, for example, unlike charges attracting and then repulsive forces being exerted on such constituents (e.g., due to like charges repelling). These factors also clearly play a large role in nucleation and/or crystal growth of the novel nanocrystals formed by affecting particle size and/or shapes; as well as permitting the crystals to be formed without the need for reductants or surfactants (i.e., that needed to be added to take part in the prior art reduction chemistry techniques) causing the nanocrystal surfaces to be free of such added chemical species. The lack of organic-based coatings on the surface of grown nanocrystals alters (and in some cases controls) their biological function.
[0464] Moreover, the particular waveform that is used for a specific frequency also affects nanocrystal growth conditions, and thus effects nanocrystal size(s) and/or shape(s). While the U.S. uses a standard AC frequency of 60 Hz, it also uses a standard waveform of a “sine” wave. As shown in the Examples herein, changing the waveform from a sine wave to a square wave or a triangular wave also affects nanocrystal crystallization conditions and thus affects resultant nanocrystal size(s) and shape(s). Preferred waveforms include sine waves, square waves and triangular waves; however hybrid waveforms should be considered to be within the metes and bounds of the invention.
[0465] Still further, the voltage applied in the novel electrochemical techniques disclosed herein can also affect nanocrystalline size(s) and shape(s). A preferred voltage range is 20-2000 Volts, a more preferred voltage range is 50-1000 Volts and an even more preferred voltage range is 100-300 Volts. In addition to voltage, the amperages used with these voltages typically are 0.1-10 Amps, a more preferred amperage range is 0.1-5 Amps and an even more preferred amperage range is 0.4-1 Amps.
[0466] Still further, the “duty cycle” used for each waveform applied in the novel electrochemical techniques disclosed herein can also affect nanocrystalline size(s) and shape(s). In this regard, without wishing to be bound by any particular theory or explanation, the amount of time that an electrode is positively biased can result in a first set of reactions, while a different set of reactions can occur when the electrode is negatively biased. By adjusting the amount of time that the electrodes are positively or negatively biased, size(s) and/or shape(s) of grown nanocrystals can be controlled. Further, the rate at which an electrode converts to + or − is also a function of waveform shape and also influences nanocrystal size(s) and/or shape(s).
[0467] Temperature can also play an important role. In some of the preferred embodiments disclosed herein, the boiling point temperature of the water is approached in at least a portion of the processing vessel where gold nanocrystals are nucleated and grown. For example, output water temperature in the continuous processing Examples herein ranges from about 60° C.-99° C. However, as discussed elsewhere herein, different temperature ranges are also desirable. Temperature can influence resultant product (e.g., size and/or shape of nanocrystals) as well as the amount of resultant product (i.e., ppm level of nanocrystals in the suspension or colloid). For example, while it is possible to cool the liquid 3 in the trough member 30 by a variety of known techniques (as disclosed in some of the Examples herein), many of the Examples herein do not cool the liquid 3, resulting in evaporation of a portion of the liquid 3 during processing thereof.
[0468]
[0469]
[0470]
[0471]
[0472]
[0473]
[0474] It should be understood that a variety of different shapes and/or cross-sections can exist for the trough member 30, any one of which can produce desirable results as a function of a variety of design and production considerations. For example, one or more constituents produced in the portion(s) 30a, 30b and/or 30c could be transient (e.g., a seed crystal or nucleation point) and/or semi-permanent (e.g., grown nanocrystals present in a colloid). If such constituent(s) produced, for example, in portion 30a is to be desirably and controllably reacted with one or more constituents produced in, for example, portion 30b, then a final product (e.g., properties of a final product) which results from such mixing could be a function of when constituents formed in the portions 30a and 30b are mixed together. Also, the temperature of liquids entering the section 30d (or 30d′) can be monitored/controlled to maximize certain desirable processing conditions and/or desirable properties of final products and/or minimize certain undesirable products. Still further, processing enhancers may be selectively utilized in one or more of the portions 30a, 30b, 30c, 30d (30d′) and/or 30o (or at any selected point or portion in the trough member 30).
[0475]
[0476]
[0477]
[0478]
[0479] Once the liquid 3 is provided into the trough member 30, means for continually moving the liquid 3 within the trough member 30 may or may not be required. However, a simple means for continually moving the liquid 3 includes the trough member 30 being situated on a slight angle θ (e.g., less than a degree to a few degrees for a low viscosity fluid 3 such as water) relative to the support surface upon which the trough member 30 is located. For example, a difference in vertical height of less than one inch between an inlet portion 31 and an outlet portion 32, spaced apart by about 6 feet (about 1.8 meters) relative to the support surface may be all that is required, so long as the viscosity of the liquid 3 is not too high (e.g., any viscosity around the viscosity of water can be controlled by gravity flow once such fluids are contained or located within the trough member 30). In this regard,
[0480]
[0481]
[0482] The electrode control devices shown generally in, for example,
[0483] First, specific reference is made to
[0484] The drive motors 21a/21b can be any suitable drive motor which is capable of small rotations (e.g., slightly below 1°/360° or slightly above 1°/360°) such that small rotational changes in the drive shaft 231a are translated into small vertical changes in the electrode assemblies. A preferred drive motor includes a drive motor manufactured by RMS Technologies model 1MC17-S04 step motor, which is a DC-powered step motor. This step motors 21a/21b include an RS-232 connection 22a/22b, respectively, which permits the step motors to be driven by a remote-control apparatus such as a computer or a controller.
[0485] The portions 271, 272 and 273 are primarily height adjustments which adjust the height of the base portion 25 relative to the trough member 30. The portions 271, 272 and 273 can be made of same, similar or different materials from the base portion 25. The portions 274a/274b and 275a/275b can also be made of the same, similar or different material from the base portion 25. However, these portions should be electrically insulating in that they house various wire components associated with delivering voltage and current to the electrode assemblies 1a/1b, 5a/5b, etc.
[0486] The electrode assembly specifically shown in
[0487] With regard to the size of the control device 20 shown in
[0488] Further, in each of the embodiments of the invention shown in
[0489]
[0490]
[0491]
[0492] In order for the control devices 20 to be actuated, two general processes need to occur. A first process involves electrically activating the electrode(s) 1 and/or 5 (e.g., applying power thereto from a preferred power source 10), and the second general process occurrence involves determining, for example, how much power is applied to the electrode(s) and appropriately adjusting electrode 1/5 height in response to such determinations (e.g., manually and/or automatically adjusting the height of the electrodes 1/5); or adjusting the electrode height or simply moving the electrode into (e.g., progressively advancing the electrode(s) 5 through the liquid 3) or out of contact with the liquid 3, as a function of time. In the case of utilizing a control device 20, suitable instructions are communicated to the step motor 21 through the RS-232 ports 22a and 22b. Important embodiments of components of the control device 20, as well as the electrode activation process, are discussed herein.
[0493] A preferred embodiment of the invention utilizes the automatic control devices 20 shown in various figures herein. The step motors 21a and 21b shown in, for example,
[0494] In particular, in this embodiment, the electrical circuit of
[0495] Each set of electrodes in Examples 1-4 of the invention has an established target voltage range. The size or magnitude of acceptable range varies by an amount between about 1% and about 10%-15% of the target voltage. Some embodiments of the invention are more sensitive to voltage changes and these embodiments should have, typically, smaller acceptable voltage ranges; whereas other embodiments of the invention are less sensitive to voltage and should have, typically, larger acceptable ranges. Accordingly, by utilizing the circuit diagram shown in
[0496] The computer or logic control for the disclosed interrogation voltage adjustment techniques are achieved by any conventional program or controller, including, for example, in a preferred embodiment, standard visual basic programming steps utilized in a PC. Such programming steps include interrogating, reading, comparing, and sending an appropriate actuation symbol to increase or decrease voltage (e.g., raise or lower an electrode relative to the surface 2 of the liquid 3). Such techniques should be understood by an artisan of ordinary skill.
[0497] Further, in another preferred embodiment of the invention utilized in Example 16 for the electrode sets 5/5′, the automatic control devices 20 are controlled by the electrical circuits of
[0498] In particular, in the Example 16 embodiments the servo-motor 21 is caused to rotate at a specific predetermined time in order to maintain a desirable electrode 5 profile. The servo-motor 21 responds by rotating a predetermined amount in a clockwise direction. Specifically the servo-motor 21 rotates a sufficient amount such that about 0.009 inches (0.229 mm) of the electrode 5 is advanced toward and into the female receiver portion o5 (shown, for example in some of
[0499] Moreover, with specific reference to
[0500] The computer or logic control for the disclosed electrode height adjustment techniques are achieved by any conventional program or controller, including, for example, in a preferred embodiment, standard visual basic programming steps utilized in a PC. Such programming steps include reading and sending an appropriate actuation symbol to lower an electrode relative to the surface 2 of the liquid 3. Such techniques should be understood by an artisan of ordinary skill.
Definitions
[0501] For purposes of the present invention, the terms and expressions below, appearing in the Specification and Claims, are intended to have the following meanings:
[0502] “Carbomer”, as used herein in Example 23, means a class of synthetically derived cross-linked polyacrylic acid polymers that provide efficient rheology modification with enhanced self-wetting for ease of use. In general, a carbomer/solvent mixture is neutralized with a base such as triethanolamine or sodium hydroxide to fully open the polymer to achieve the desired thickening, suspending, and emulsion stabilization properties to make creams or gels.
[0503] “Substantially clean”, as used herein should be understood when used to describe nanocrystal surfaces means that the nanocrystals do not have chemical constituents adhered or attached to their surfaces in such an amount that would materially alter the functioning of the nanocrystal in at least one of its significant properties of the gold nanocrystals set forth in the Examples herein. Alternatively, the gold nanocrystal does not have a layer, surface or film which covers a significant portion (e.g., at least 25% of the crystal, or in another embodiment at least 50% of the crystal). It also can mean that the nanocrystal surfaces are completely free of any organic contaminants which materially change their functionality over bare gold crystal surfaces. It should be understood that incidental components that are caused to adhere to nanocrystals of the invention and do not adversely or materially affect the functioning of the inventive nanocrystals, should still be considered to be within the metes and bounds of the invention. The term should also be understood to be a relative term referencing the lack of traditional organic-based molecules (i.e., those used in traditional reduction chemistry techniques) on the surfaces of the grown nanocrystals of the invention.
[0504] A “diagnostic effective amount”, as used herein, means an amount sufficient to bind to MIF to enable detection of the MIF-compound complex such that diagnosis of a disease or condition is possible.
[0505] An “effective amount”, as used herein, means a certain amount of solution or compound which, when administered according to, for example, a desired dosing regimen, provides the desired MIF cytokine inhibiting or treatment or therapeutic activity, or disease/condition prevention or MIF signaling pathway(s). Dosing may occur at intervals of minutes, hours, days, weeks, months or years or continuously over any one of these periods.
[0506] As used herein, “immune privilege” refers to an area or site within a living system (e.g., a body) which tolerates the presence of an antigen that would normally elicit a response from the immune system (e.g., an inflammatory immune response).
[0507] The term “operably coating” a stent means coating a stent in a way that permits the timely release of the inventive metallic-based nanocrystals (e.g., comprising aqueous gold-based metal and/or mixtures of gold and other metal(s) and/or alloys of gold with other metal(s)) into the surrounding tissue to be treated once the coated stent is administered.
[0508] As used herein, the term “processing-enhancer” or “processing-enhanced” or “process enhancer” means at least one material (e.g., solid, liquid and/or gas) and typically means an inorganic material, which material does not significantly bind to the formed nanocrystals, but rather facilitates nucleation/growth during an electrochemical-stimulated growth process. The material serves important roles in the process including providing charged ions in the electrochemical solution to permit the crystals to be grown. The process enhancer is critically a compound(s) which remains in solution, and/or does not form a coating (in one embodiment an organic coating), and/or does not adversely affect the formed nanocrystals or the formed suspension(s), and/or is destroyed, evaporated, or is otherwise lost during the electrochemical crystal growth process.
[0509] The term “Steroid-sparing”, as used herein, means providing a material other than a steroid in a combination therapy which reduces the amount of steroid required to be effective for treating/preventing an indication.
[0510] The phrase “trough member” as used herein should be understood as meaning a large variety of fluid handling devices including, pipes, half pipes, channels or grooves existing in materials or objects, conduits, ducts, tubes, chutes, hoses and/or spouts, so long as such are compatible with the electrochemical processes disclosed herein.
[0511] The following Examples serve to illustrate certain embodiments of the invention but should not to be construed as limiting the scope of the disclosure as defined in the appended claims.
Examples 1-4
Manufacturing Gold-Based Nanoparticles/Nanoparticle Solutions GT032, GT031, GT019 and GT033
[0512] In general, each of Examples 1-4 utilizes certain embodiments of the invention associated with the apparatuses generally shown in
[0513] Purified water (discussed later herein) was used as the input liquid 3 in Example 1. In Examples 2-4, a processing enhancer was added to the liquid 3 being input into the trough member 30. The specific processing enhancer added, as well as the specific amounts of the same, were effective in these examples. However, other processing enhancer(s) and amounts of same, should be viewed as being within the metes and bounds of this disclosure and these specific examples should not be viewed as limiting the scope of the invention. The depth “d” (refer to
[0514] The rate of flow of the water 3 into the trough member 30 was about 90 ml/minute. Due to some evaporation within the trough member 30, the flow out of the trough member 30 was slightly less, about 60-70 ml/minute. Such flow of water 3 into the trough member 30 was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 90 milliliters per minute. Tygon® tubing having a diameter of ¼″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30 by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30 as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30 such that when the reservoir overflowed, a relatively steady flow of water 3 into the end 31 of the V-shaped trough member 30 occurred.
[0515] With regard to
[0516] The power source for each electrode set was an AC transformer 60. Specifically,
[0517] When a secondary coil 603 is positioned near the primary coil 601 and core 602, this flux will link the secondary coil 603 with the primary coil 601. This linking of the secondary coil 603 induces a voltage across the secondary terminals. The magnitude of the voltage at the secondary terminals is related directly to the ratio of the secondary coil turns to the primary coil turns. More turns on the secondary coil 603 than the primary coil 601 results in a step up in voltage, while fewer turns results in a step down in voltage.
[0518] Preferred transformer(s) 60 for use in these Examples have deliberately poor output voltage regulation made possible by the use of magnetic shunts in the transformer 60. These transformers 60 are known as neon sign transformers. This configuration limits current flow into the electrode(s) 1/5. With a large change in output load voltage, the transformer 60 maintains output load current within a relatively narrow range.
[0519] The transformer 60 is rated for its secondary open circuit voltage and secondary short circuit current. Open circuit voltage (OCV) appears at the output terminals of the transformer 60 only when no electrical connection is present. Likewise, short circuit current is only drawn from the output terminals if a short is placed across those terminals (in which case the output voltage equals zero). However, when a load is connected across these same terminals, the output voltage of the transformer 60 should fall somewhere between zero and the rated OCV. In fact, if the transformer 60 is loaded properly, that voltage will be about half the rated OCV.
[0520] The transformer 60 is known as a Balanced Mid-Point Referenced Design (e.g., also formerly known as balanced midpoint grounded). This is most commonly found in mid to higher voltage rated transformers and most 60 mA transformers. This is the only type transformer acceptable in a “mid-point return wired” system. The “balanced” transformer 60 has one primary coil 601 with two secondary coils 603, one on each side of the primary coil 601 (as shown generally in the schematic view in
[0521] In alternating current (AC) circuits possessing a line power factor or 1 (or 100%), the voltage and current each start at zero, rise to a crest, fall to zero, go to a negative crest and back up to zero. This completes one cycle of a typical sine wave. This happens 60 times per second in a typical US application. Thus, such a voltage or current has a characteristic “frequency” of 60 cycles per second (or 60 Hertz) power. Power factor relates to the position of the voltage waveform relative to the current waveform. When both waveforms pass through zero together and their crests are together, they are in phase and the power factor is 1, or 100%.
[0522] The normal power factor of most such transformers 60 is largely due to the effect of the magnetic shunts 604 and the secondary coil 603, which effectively add an inductor into the output of the transformer's 60 circuit to limit current to the electrodes 1/5. The power factor can be increased to a higher power factor by the use of capacitor(s) 61 placed across the primary coil 601 of the transformer, 60 which brings the input voltage and current waves more into phase.
[0523] The unloaded voltage of any transformer 60 to be used in the present invention is important, as well as the internal structure thereof. Desirable unloaded transformers for use in the present invention include those that are around 9,000 volts, 10,000 volts, 12,000 volts and 15,000 volts. However, these particular unloaded volt transformer measurements should not be viewed as limiting the scope acceptable power sources as additional embodiments. A specific desirable transformer for use in these Examples is made by Franceformer, Catalog No. 9060-P-E which operates at: primarily 120 volts, 60 Hz; and secondary 9,000 volts, 60 mA.
[0524]
[0525]
[0526]
[0527]
[0528] Accordingly, each transformer assembly 60a-60h (and/or 60a′-60h′; and/or 60a″-60h″) can be the same transformer, or can be a combination of different transformers (as well as different polarities). The choice of transformer, power factor, capacitor(s) 61, polarity, electrode designs, electrode location, electrode composition, cross-sectional shape(s) of the trough member 30, local or global electrode composition, atmosphere(s), local or global liquid 3 flow rate(s), liquid 3 local components, volume of liquid 3 locally subjected to various fields in the trough member 30, neighboring (e.g., both upstream and downstream) electrode sets, local field concentrations, the use and/or position and/or composition of any membrane used in the trough member, etc., are all factors which influence processing conditions as well as composition and/or volume of constituents produced in the liquid 3, nanocrystals and nanocrystal/suspensions or colloids made according to the various embodiments disclosed herein. Accordingly, a plethora of embodiments can be practiced according to the detailed disclosure presented herein.
[0529] The size and shape of each electrode 1 utilized was about the same. The shape of each electrode 1 was that of a right triangle with measurements of about 14 mm×23 mm×27 mm. The thickness of each electrode 1 was about 1 mm. Each triangular-shaped electrode 1 also had a hole therethrough at a base portion thereof, which permitted the point formed by the 23 mm and 27 mm sides to point toward the surface 2 of the water 3. The material comprising each electrode 1 was 99.95% pure (i.e., 3N5) unless otherwise stated herein. When gold was used for each electrode 1, the weight of each electrode was about 9 grams.
[0530] The wires used to attach the triangular-shaped electrode 1 to the transformer 60 were, for Examples 1-3, 99.95% (3N5) platinum wire, having a diameter of about 1 mm.
[0531] The wires used for each electrode 5 comprised 99.95% pure (3N5) gold each having a diameter of about 0.5 mm. All materials for the electrodes 1/5 were obtained from ESPI having an address of 1050 Benson Way, Ashland, Oreg. 97520.
[0532] The water 3 used in Example 1 as an input into the trough member 30 (and used in Examples 2-4 in combination with a processing enhancer) was produced by a Reverse Osmosis process and deionization process. In essence, Reverse Osmosis (RO) is a pressure driven membrane separation process that separates species that are dissolved and/or suspended substances from the ground water. It is called “reverse” osmosis because pressure is applied to reverse the natural flow of osmosis (which seeks to balance the concentration of materials on both sides of the membrane). The applied pressure forces the water through the membrane leaving the contaminants on one side of the membrane and the purified water on the other. The reverse osmosis membrane utilized several thin layers or sheets of film that are bonded together and rolled in a spiral configuration around a plastic tube. (This is also known as a thin film composite or TFC membrane.) In addition to the removal of dissolved species, the RO membrane also separates out suspended materials including microorganisms that may be present in the water. After RO processing a mixed bed deionization filter was used. The total dissolved solvents (“TDS”) after both treatments was about 0.2 ppm, as measured by an Accumet® AR20 pH/conductivity meter.
[0533] These examples use gold electrodes for the 8 electrode sets. In this regard, Tables 1a-1d set forth pertinent operating parameters associated with each of the 16 electrodes in the 8 electrode sets utilized to make gold-based nanocrystals/nanocrystal suspensions.
TABLE-US-00003 TABLE 1a Cold Input Water (Au) Run ID: GT032 Flow Rate: 90 ml/min Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 0.4 Zeta: n/a Target Distance Distance Average Elec- Voltage “c-c” “x” Voltage Set # trode # (kV) in/mm in/mm (kV) 7/177.8* 1 1a 1.6113 0.22/5.59 1.65 5a 0.8621 N/A 0.84 8/203.2 2 5b 0.4137 N/A 0.39 .sup. 5b′ 0.7679 N/A 0.76 8/203.2 3 5c 0.491 N/A 0.49 .sup. 5c′ 0.4816 N/A 0.48 8/203.2 4 1d 0.4579 N/A 0.45 5d 0.6435 N/A 0.6 9/228.6 5 5e 0.6893 N/A 0.67 .sup. 5e′ 0.2718 N/A 0.26 8/203.2 6 5f 0.4327 N/A 0.43 .sup. 5f′ 0.2993 N/A 0.3 8/203.2 7 5g 0.4691 N/A 0.43 .sup. 5g′ 0.4644 N/A 0.46 8/203.2 8 5h 0.3494 N/A 0.33 .sup. 5h′ 0.6302 N/A 0.61 8/203.2** Output Water Temperature 65 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water outlet
TABLE-US-00004 TABLE 1b .0383 mg/mL of NaHCO.sub.3 (Au) Run ID: GT031 Flow Rate: 90 ml/min NaHCO.sub.3: 0.038 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 1.5 Zeta: n/a Target Distance Distance Average Elec- Voltage “c-c” “x” Voltage Set # trode # (kV) in/mm in/mm (kV) 7/177.8* 1 1a 1.7053 0.22/5.59 1.69 5a 1.1484 N/A 1.13 8/203.2 2 5b 0.6364 N/A 0.63 .sup. 5b′ 0.9287 N/A 0.92 8/203.2 3 5c 0.7018 N/A 0.71 .sup. 5c′ 0.6275 N/A 0.62 8/203.2 4 5d 0.6798 N/A 0.68 5d 0.7497 N/A 0.75 9/228.6 5 5e 0.8364 N/A 0.85 .sup. 5e′ 0.4474 N/A 0.45 8/203.2 6 5f 0.5823 N/A 0.59 .sup. 5f′ 0.4693 N/A 0.47 8/203.2 7 5g 0.609 N/A 0.61 .sup. 5g′ 0.5861 N/A 0.59 8/203.2 8 5h 0.4756 N/A 0.48 .sup. 5h′ 0.7564 N/A 0.76 8/203.2** Output Water Temperature 64 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water outlet
TABLE-US-00005 TABLE 1c .045 mg/ml of NaCl (Au) Run ID: GT019 Flow Rate: 90 ml/min NaCl: .045 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 6.1 Zeta: n/a Target Distance Distance Average Elec- Voltage “c-c” “x” Voltage Set # trode # (kV) in/mm in/mm (kV) 7/177.8* 1 1a 1.4105 0.22/5.59 1.41 5a 0.8372 N/A 0.87 8/203.2 2 5b 0.3244 N/A 0.36 .sup. 5b′ 0.4856 N/A 0.65 8/203.2 3 5c 0.3504 N/A 0.37 .sup. 5c′ 0.3147 N/A 0.36 8/203.2 4 5d 0.3526 N/A 0.37 5d 0.4539 N/A 0.5 9/228.6 5 5e 0.5811 N/A 0.6 .sup. 5e′ 0.2471 N/A 0.27 8/203.2 6 5f 0.3624 N/A 0.38 .sup. 5f′ 0.2905 N/A 0.31 8/203.2 7 5g 0.3387 N/A 0.36 .sup. 5g′ 0.3015 N/A 0.33 8/203.2 8 5h 0.2995 N/A 0.33 .sup. 5h′ 0.5442 N/A 0.57 8/203.2** Output Water Temperature 77 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water outlet
TABLE-US-00006 TABLE 1d .038 mg/mL of NaHCO.sub.3 (Au) Run ID: GT033 Flow Rate: 90 ml/min NaHCO.sub.3: 0.038 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 2.0 Zeta: n/a Target Distance Distance Average Elec- Voltage “c-c” “x” Voltage Set # trode # (kV) in/mm in/mm (kV) 7/177.8* 1 1a 1.6033 0.22/5.59 1.641826 5a 1.1759 N/A 1.190259 8/203.2 2 5b 0.6978 N/A 0.727213 .sup. 5b′ 0.8918 N/A 0.946323 8/203.2 3 5c 0.6329 N/A 0.795378 .sup. 5c′ 0.526 N/A 0.609542 8/203.2 4 5d 0.609 N/A 0.613669 5d 0.6978 N/A 0.719777 9/228.6 5 5e 0.9551 N/A 0.920594 .sup. 5e′ 0.5594 N/A 0.547233 8/203.2 6 5f 0.6905 N/A 0.657295 .sup. 5f′ 0.5516 N/A 0.521984 8/203.2 7 5g 0.5741 N/A 0.588502 .sup. 5g′ 0.5791 N/A 0.541565 8/203.2 8 5h 0.4661 N/A 0.46091 .sup. 5h′ 0.7329 N/A 0.741009 8/203.2** Output Water Temperature 83 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water outlet
[0534] Table 1a shows that a “1/5” electrode configuration was utilized for Electrode Set #1 and for Electrode Set #4, and all other sets were of the 5/5 configuration; whereas Tables 1b, 1c and 1d show that Electrode Set #1 was the only electrode set utilizing the 1/5 configuration, and all other sets were of the 5/5 configuration.
[0535] Additionally, the following differences in manufacturing set-up were also utilized:
[0536] Example 1: GT032: The input water 3 into the trough member 30 was chilled in a refrigerator unit until it reached a temperature of about 2° C. and was then pumped into the trough member 30;
[0537] Example 2: GT031: A processing enhancer was added to the input water 3 prior to the water 3 being input into the trough member 30. Specifically, about 0.145 grams/gallon (i.e., about 38.3 mg/liter) of sodium hydrogen carbonate (“soda”), having a chemical formula of NaHCO.sub.3, was added to and mixed with the water 3. The soda was obtained from Alfa Aesar and the soda had a formula weight of 84.01 and a density of about 2.159 g/cm.sup.3 (i.e., stock #14707, lot D15T043).
[0538] Example 3: GT019: A processing enhancer was added to the input water 3 prior to the water 3 being input into the trough member 30. Specifically, about 0.17 grams/gallon (i.e., about 45 mg/liter) of sodium chloride (“salt”), having a chemical formula of NaCl, was added to and mixed with the water 3.
[0539] Example 4: GT033: A processing enhancer was added to the input water 3 prior to the water 3 being input into the trough member 30. Specifically, about 0.145 grams/gallon (i.e., about 38.3 mg/liter) of sodium hydrogen carbonate (“soda”), having a chemical formula of NaHCO.sub.3, was added to and mixed with the water 3. The soda was obtained from Alfa Aesar and the soda had a formula weight of 84.01 and a density of about 2.159 g/cm.sup.3 (i.e., stock #14707, lot D15T043). A representative TEM photomicrograph of dried solution GT033 is shown in
[0540] The salt used in Example 3 was obtained from Fisher Scientific (lot #080787) and the salt had a formula weight of 58.44 and an actual analysis as follows:
TABLE-US-00007 Assay .sup. 100% Barium (BA) Pass Test Bromide <0.010% Calcium 0.0002% Chlorate & Nitrate <0.0003% Heavy Metals (AS PB) <5.0 ppm Identification Pass Test Insoluble Water <0.001% Iodide 0.0020% Iron (FE) <2.0 ppm Magnesium <0.0005% Ph 5% Soln @ 25 Deg C. 5.9 Phosphate (PO4) <5.0 ppm Potassium (K) <0.003% Sulfate (SO4) <0.0040%
[0541] Table 1e summarizes the physical characteristics results for each of the three suspensions GT032, GT031 and GT019. Full characterization of GT019 was not completed, however, it is clear that under the processing conditions discussed herein, both processing enhancers (i.e., soda and salt) increase the measured ppm of gold in the suspensions GT031 and GT019 relative to GT032.
TABLE-US-00008 TABLE 1e Zeta Predominant Poten- DLS DLS Mass Color tial % Trans- Distribution Peak of Sus- PPM (Avg) pH mission (Radius in nm) pension GT032 0.4 −19.30 3.29 11.7% 3.80 Clear GT031 1.5 −29.00 5.66 17.0% 0.78 Purple GT019 6.1 ** ** ** ** Pink GT033 2.0 ** ** .sup. 30% ** Pink ** Values not measured
Examples 5-7
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspensions GD-007, GD-016 and GD-015
[0542] In general, each of Examples 5-7 utilize certain embodiments of the invention associated with the apparatuses generally shown in
[0543] Purified water (discussed elsewhere herein) was mixed with about 0.396 g/L of NaHCO.sub.3 and was used as the liquid 3 input into trough member 30a. While the amount of NaHCO.sub.3 used was effective, this amount should not be viewed as limiting the metes and bounds of the invention, and other amounts are within the metes and bounds of this disclosure. The depth “d” (refer to
[0544] The rate of flow of the water 3 into the trough member 30a was about 150 ml/minute (note: there was minimal evaporation in the trough member 30a). Such flow of water 3 into the trough member 30a was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 150 milliliters per minute. Tygon® tubing having a diameter of 1/4″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30a by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30a as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30a such that when the reservoir overflowed, a relatively steady flow of water 3 into the end 31 of the V-shaped trough member 30a occurred.
[0545] There were 5 electrode sets used in Examples 5-7 and one set was a single electrode set 1a/5a located in trough member 30a. The plasma 4 in trough member 30a from electrode 1a was created with an electrode 1a similar in shape to that shown in
[0546] The output of the processing-enhanced, conditioned water 3′ was collected into a reservoir 41 and subsequently pumped by another pump 40′ into a second trough member 30b, at substantially the same rate as pump 40 (e.g., minimal evaporation occurred in trough member 30a). The second trough member 30b measured about 30 inches long by 1.5 inches wide by 5.75 inches high and contained about 2500 ml of water 3″ therein. Each of four electrode sets 5b, 5b′-5e, 5e′ comprised 99.95% pure gold wire measuring about 0.5 mm in diameter and about 5 inches (about 12 cm) in length and was substantially straight. About 4.25 inches (about 11 cm) of wire was submerged in the water 3″ which was about 4.5 inches (about 11 cm) deep.
[0547] With regard to
[0548] Each of Tables 2a-2c contains processing information relating to each of the 4 electrode sets in trough 30b by “Set #”. Each electrode of the 4 electrode sets in trough 30b was set to operate at a specific target voltage. Actual operating voltages of about 255 volts, as listed in each of Tables 2a-2c, were applied across the electrode sets. The distance “c-c” (with reference to
[0549] All materials for the electrodes 1/5 were obtained from ESPI having an address of 1050 Benson Way, Ashland, Oreg. 97520.
[0550] The water 3 used in Examples 5-7 was produced by a Reverse Osmosis process and deionization process and was mixed with the NaHCO.sub.3 processing-enhancer and together was input into the trough member 30a. In essence, Reverse Osmosis (RO) is a pressure driven membrane separation process that separates species that are dissolved and/or suspended substances from the ground water. It is called “reverse” osmosis because pressure is applied to reverse the natural flow of osmosis (which seeks to balance the concentration of materials on both sides of the membrane). The applied pressure forces the water through the membrane leaving the contaminants on one side of the membrane and the purified water on the other. The reverse osmosis membrane utilized several thin layers or sheets of film that are bonded together and rolled in a spiral configuration around a plastic tube. (This is also known as a thin film composite or TFC membrane.) In addition to the removal of dissolved species, the RO membrane also separates out suspended materials including microorganisms that may be present in the water. After RO processing a mixed bed deionization filter was used. The total dissolved solvents (“TDS”) after both treatments was about 0.2 ppm, as measured by an Accumet® AR20 pH/conductivity meter.
TABLE-US-00009 TABLE 2a 0.396 mg/ml of NaHCO.sub.3 (Au) Run ID: GD-007 Flow Rate: 150 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 14.8 Zeta: n/a Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 8.5/215.9 3 5c N/A 255 Rectangle .sup. 5c′ N/A 5.25″ 8.5/215.9 Deep 4 5d N/A 255 .sup. 5d′ N/A .sup. 8/203.2 5 5e N/A 255 .sup. 5e′ N/A 2/50.8** Output Water Temperature 96 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
TABLE-US-00010 TABLE 2b 0.396 mg/ml of NaHCO.sub.3 (Au) Run ID: GD-016 Flow Rate: 150 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 12.5 Zeta: −56.12 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 8.5/215.9 3 5c N/A 255 Rectangle .sup. 5c′ N/A 5.25″ 8.5/215.9 Deep 4 5d N/A 255 .sup. 5d′ N/A .sup. 8/203.2 5 5e N/A 255 .sup. 5e′ N/A 2/50.8** Output Water Temperature 97 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
TABLE-US-00011 TABLE 2c 0.396 mg/ml of NaHCO3 (Au) Run ID: GD-015 Flow Rate: 150 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 14.5 Zeta: −69.1 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 8.5/215.9 3 5c N/A 255 Rectangle .sup. 5c′ N/A 5.25″ 8.5/215.9 Deep 4 5d N/A 255 .sup. 5d′ N/A .sup. 8/203.2 5 5e N/A 255 .sup. 5e′ N/A 2/50.8** Output Water Temperature 96 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
[0551] Representative Transmission Electron Microscopy (TEM) photomicrographs (
Transmission Electron Microscopy
[0552] Specifically, TEM samples were prepared by utilizing a Formvar coated grid stabilized with carbon having a mesh size of 200. The grids were first pretreated by a plasma treatment under vacuum. The grids were placed on a microscope slide lined with a rectangular piece of filter paper and then placed into a Denton Vacuum apparatus with the necessary plasma generator accessory installed. The vacuum was maintained at 75 mTorr and the plasma was initiated and run for about 30 seconds. Upon completion, the system was vented, and the grids removed. The grids were stable up to 7-10 days depending upon humidity conditions, but in all instances were used within 12 hours.
[0553] Approximately 1 μL of each inventive nanocrystal suspension was placed onto each grid and was allowed to air dry at room temperature for 20-30 minutes, or until the droplet evaporated. Upon complete evaporation, the grids were placed onto a holder plate until TEM analysis was performed.
[0554] A Philips/FEI Tecnai 12 Transmission Electron Microscope was used to interrogate all prepared samples. The instrument was run at an accelerating voltage of 100 keV. After alignment of the beam, the samples were examined at various magnifications up to and including 630,000×. Images were collected via the attached Olympus Megaview III side-mounted camera that transmitted the images directly to a PC equipped with iTEM and Tecnai User Interface software which provided for both control over the camera and the TEM instrument, respectively.
[0555] Within the iTEM software, it was possible to randomly move around the grid by adjusting the position of a crosshair on a circular reference plane. By selecting and moving the cross-hairs, one could navigate around the grid. Using this function, the samples were analyzed at four quadrants of the circular reference, allowing for an unbiased representation of the sample. The images were later analyzed with ImageJ 1.42 software. Another similar software program which measured the number of pixels across each particle relative to a known number of pixels in a spacer bar was used to streamline the particle counting process. The particles were measured using the scale bar on the image as a method to calibrate the software prior to measuring each individual particle. Once calibrated, particles were measured based upon the following parameters: Tetrahedral particles were measured from the triangle's apex to the base. Pentagonal bipyramids were measured from either apex to apex of the diamond or apex of the pentagon to the base of the pentagon depending upon the particle orientation on the grid. Icosahedrons were measured using the longest distance between two faces of a hexagonal particle. Spherical or irregular shaped particles were measured along the longest axis. The data collected from each sample set was exported to Excel, and using a simple histogram function with 50 bins with a minimum of 5 nm and maximum of 50 nm, a histogram was generated. Subsequently, the data generated within Excel was exported to Prism (GraphPad™) and fit to one of two models, a normal distribution or log normal distribution, each having a unique probability density function (PDF). Within Prism, it was possible to analyze the histogram data by performing a non-linear fit to the data which generates a distribution known as a normal distribution. Moreover, it was possible to perform a logarithmic transformation on the non-linear data set to generate a data set that is then fit to a non-linear model and then transformed via an exponential transformation to generate a log-normal fit of the data. The two models were then visually compared to the histogram and the model that fit the data to a better degree was chosen. The particle diameter noted above, and reported in the many Histogram Figures and Tables herein, is the mode of the PDF, which is defined as the maximum value of the log-normal or normal PDF curve. This PDF curve is overlaid on all histogram figures wherein the mode value is displayed directly above and is referenced in text as the TEM average diameter.
[0556] For example,
[0557]
[0558] The results shown in
[0559]
[0560]
[0561] Further, dynamic light scattering techniques were also utilized to obtain an indication of crystal sizes (e.g., hydrodynamic radii) produced according to the Examples herein.
Dynamic Light Scattering
[0562] Specifically, dynamic light scattering (DLS) measurements were performed on Viscotek 802 DLS instrument. In DLS, as the laser light hits small particles and/or organized water structures around the small particles (smaller than the wavelength), the light scatters in all directions, resulting in a time-dependent fluctuation in the scattering intensity. Intensity fluctuations are due to the Brownian motion of the scattering particles/water structure combination and contain information about the crystal size distribution.
[0563] The instrument was allowed to warm up for at least 30 min prior to the experiments. The measurements were made using 12 μl quartz cell. The following procedure was used: [0564] 1. First, 1 ml of DI water was added into the cell using 1 ml micropipette, then water was poured out of the cell to a waste beaker and the rest of the water was shaken off the cell measuring cavity. This step was repeated two more times to thoroughly rinse the cell. [0565] 2. 100 μl of the sample was added into the cell using 200 μl micropipette. After that all liquid was removed out of the cell with the same pipette using the same pipette tip and expelled into the waste beaker. 100 μl of the sample was added again using the same tip. [0566] 3. The cell with the sample was placed into a temperature-controlled cell block of the Viscotek instrument with frosted side of the cell facing left. A new experiment in Viscotek OmniSIZE software was opened. The measurement was started Imin after the temperature equilibrated and the laser power attenuated to the proper value. The results were saved after all runs were over. [0567] 4. The cell was taken out of the instrument and the sample was removed out of the cell using the same pipette and the tip used if step 2. [0568] 5. Steps 2 to 4 were repeated two more times for each sample. [0569] 6. For a new sample, a new pipette tip for 200 μl pipette was taken to avoid contamination with previous sample and steps 1 through 5 were repeated.
[0570] Data collection and processing was performed with OmniSIZE software, version 3,0,0,291. The following parameters were used for all the experiments: Run Duration—3s; Experiments—100; Solvent—water, 0 mmol; Viscosity—1 cP; Refractive Index—1.333; Spike Tolerance—20%; Baseline Drift—15%; Target Attenuation—300k Counts; block temperature—+40° C. After data for each experiment were saved, the results were viewed on “Results” page of the software. Particle size distribution (i.e., hydrodynamic radii) was analyzed in “Intensity distribution” graph. On that graph any peaks outside of 0.1 nm-10 μm range were regarded as artifacts. Particularly, clean water (no particles) results no peaks within 0.1 nm-10 μm range and a broad peak below 0.1 nm. This peak is taken as a noise peak (noise flow) of the instrument. Samples with very low concentration or very small size of suspended nanocrystals or nanoparticles may exhibit measurable noise peak in “Intensity distribution” graph. If the peaks within 0.1 nm-10 μm range have higher intensity than the noise peak, those peaks considered being real, otherwise the peaks are questionable and may represent artifacts of data processing.
[0571]
[0572] It should be noted that the dynamic light scattering particle size information is different from the TEM measured histograms because dynamic light scattering uses algorithms that assume the nanocrystals are all spheres (which they are not) as well as measures the hydrodynamic radius (e.g., the nanocrystal's influence on the water is also detected and reported in addition to the actual physical radii of the particles). Accordingly, it is not surprising that there is a difference in the reported particle sizes between those reported in the TEM histogram data and those reported in the dynamic light scattering data, just as in the other Examples included herein.
Atomic Absorption Spectroscopy
[0573] The AAS values were obtained from a Perkin Elmer Analyst 400 Spectrometer system.
I) Principle
[0574] The technique of flame atomic absorption spectroscopy requires a liquid sample to be aspirated, aerosolized and mixed with combustible gases, such as acetylene and air. The mixture is ignited in a flame whose temperature ranges from about 2100 to about 2400 degrees C. During combustion, atoms of the element of interest in the sample are reduced to free, unexcited ground state atoms, which absorb light at characteristic wavelengths. The characteristic wavelengths are element specific and are accurate to 0.01-0.1 nm. To provide element specific wavelengths, a light beam from a hollow cathode lamp (HCL), whose cathode is made of the element being determined, is passed through the flame. A photodetector detects the amount of reduction of the light intensity due to absorption by the analyte. A monochromator is used in front of the photodetector to reduce background ambient light and to select the specific wavelength from the HCL required for detection. In addition, a deuterium arc lamp corrects for background absorbance caused by non-atomic species in the atom cloud.
II) Sample Preparation
[0575] 10 mL of sample, 0.6 mL of 36% v/v hydrochloric acid and 0.15 mL of 50% v/v nitric acid are mixed together in a glass vial and incubated for about 10 minutes in 70 degree C. water bath. If gold concentration in the suspension is expected to be above 10 ppm a sample is diluted with DI water before addition of the acids to bring final gold concentration in the range of 1 to 10 ppm. For example, for a gold concentration around 100 ppm, 0.5 mL of sample is diluted with 9.5 mL of DI water before the addition of acids. Aliquoting is performed with adjustable micropipettes and the exact amount of sample, DI water and acids is measured by an Ohaus PA313 microbalance. The weights of components are used to correct measured concentration for dilution by DI water and acids. [0576] Each sample is prepared in triplicate and after incubation in water bath is allowed to cool down to room temperature before measurements are made.
III) Instrument Setup
[0577] The following settings are used for Perkin Elmer Analyst 400 Spectrometer system: [0578] a) Burner head: 10 cm single-slot type, aligned in three axes according to the manufacture procedure to obtain maximum absorbance with a 2 ppm Cu standard. [0579] b) Nebulizer: plastic with a spacer in front of the impact bead. [0580] c) Gas flow: oxidant (air) flow rate about 12 L/min, fuel (acetylene) flow rate about 1.9 mL/min. [0581] d) Lamp/monochromator: Au hollow cathode lamp, 10 mA operating current, 1.8/1.35 mm slits, 242.8 nm wavelength, background correction (deuterium lamp) is on.
IV) Analysis Procedure
[0582] a) Run the Au lamp and the flame for approximately 30 minutes to warm up the system. [0583] b) Calibrate the instrument with 1 ppm, 4 ppm and 10 ppm Au standards in a matrix of 3.7% v/v hydrochloric acid. Use 3.7% v/v hydrochloric acid as a blank. [0584] c) Verify calibration scale by measuring 4 ppm standard as a sample. The measured concentration should be between 3.88 ppm and 4.12 ppm. Repeat step b) if outside that range. [0585] d) Measure three replicas of a sample. If the standard deviation between replicas is higher than 5%, repeat measurement, otherwise proceed to the next sample. [0586] e) Perform verification step c) after measuring six samples or more often. If verification fails, perform steps b) and c) and remeasure all the samples measured after the last successful verification.
V) Data Analysis
[0587] Measured concentration value for each replica is corrected for dilution by water and acid to calculate actual sample concentration. The reported Au ppm value is the average of three corrected values for individual replica.
Plasma Irradiance and Characterization
[0588] This Example provides a spectrographic analysis of the adjustable plasmas 4, utilizing a gold electrode 1, all of which were utilized in the Examples herein. Three different spectrometers with high sensitivities were used to collect spectral information about the plasmas 4. Specifically, spectrographic analysis was conducted on several gold electrode plasmon. The species in the plasmas 4, as well as different intensities of some of the species, were observed. The presence/absence of such species can affect (e.g., positively and negatively) processing parameters and products made according to the teachings herein.
[0589] In this regard,
[0590] Specifically, the experimental setup for collecting plasma emission data (e.g., irradiance) is depicted in
[0591] The assembly 524 contained one UV collimator (LC-10U) with a refocusing assembly (LF-10U100) for the 170-2400 nm range. The assembly 524 also included an SMA female connector made by Multimode Fiber Optics, Inc. Each LC-10U and LF-10U100 had one UV fused silica lens associated therewith. Adjustable focusing was provided by LF-10U100 at about 100 mm from the vortex of the lens in LF-10U100 also contained in the assembly 524.
[0592] The collimator field of view at both ends of the adjustable plasma 4 was about 1.5 mm in diameter as determined by a 455 μm fiber core diameter comprising the solarization resistant UV optical fiber 523 (180-900 nm range and made by Mitsubishi). The UV optical fiber 523 was terminated at each end by an SMA male connector (sold by Ocean Optics; QP450-1-XSR).
[0593] The UV collimator-fiber system 523 and 524 provided 180-900 nm range of sensitivity for plasma irradiance coming from the 1.5 mm diameter plasma cylinder horizontally oriented in different locations in the adjustable plasma 4.
[0594] The X-Z stage 525 comprised two linear stages (PT1) made by Thorlabs Inc., that hold and control movement of the UV collimator 524 along the X and Z axes. It is thus possible to scan the adjustable plasma 4 horizontally and vertically, respectively.
[0595] Emission of plasma radiation collected by UV collimator-fiber system 523, 524 was delivered to either of three fiber coupled spectrometers 520, 521 or 522 made by StellarNet, Inc. (i.e., EPP2000-HR for 180-295 nm, 2400 g/mm grating, EPP2000-HR for 290-400 nm, 1800 g/mm grating, and EPP2000-HR for 395-505 nm, 1200 g/mm grating). Each spectrometer 520, 521 and 522 had a 7 μm entrance slit, 0.1 nm optical resolution and a 2048-pixel CCD detector. Measured instrumental spectral line broadening is 0.13 nm at 313.1 nm.
[0596] Spectral data acquisition was controlled by SpectraWiz software for Windows/XP made by StellarNet. All three EPP2000-HR spectrometers 520, 521 and 522 were interfaced with one personal computer 528 equipped with 4 USB ports. The integration times and number of averages for various spectral ranges and plasma discharges were set appropriately to provide unsaturated signal intensities with the best possible signal to noise ratios. Typically, spectral integration time was order of 1 second and number averaged spectra was in range 1 to 10. All recorded spectra were acquired with subtracted optical background. Optical background was acquired before the beginning of the acquisition of a corresponding set of measurements each with identical data acquisition parameters.
[0597] Each UV fiber-spectrometer system (i.e., 523/520, 523/521 and 523/522) was calibrated with an AvaLight-DH-CAL Irradiance Calibrated Light Source, made by Avantes (not shown). After the calibration, all acquired spectral intensities were expressed in (absolute) units of spectral irradiance (mW/m.sup.2/nm), as well as corrected for the nonlinear response of the UV-fiber-spectrometer. The relative error of the AvaLight-DH-CAL Irradiance Calibrated Light Source in 200-1100 nm range is not higher than 10%.
[0598] Alignment of the field of view of the UV collimator assembly 524 relative to the tip 9 of the metal electrode 1 was performed before each set of measurements. The center of the UV collimator assembly 524 field of view was placed at the tip 9 by the alignment of two linear stages and by sending a light through the UV collimator-fiber system 523, 524 to the center of each metal electrode 1.
[0599] The X-Z stage 525 was utilized to move the assembly 524 into roughly a horizontal, center portion of the adjustable plasma 4, while being able to move the assembly 524 vertically such that analysis of the spectral emissions occurring at different vertical heights in the adjustable plasma 4 could be made. In this regard, the assembly 524 was positioned at different heights, the first of which was located as close as possible of the tip 9 of the electrode 1, and thereafter moved away from the tip 9 in specific amounts. The emission spectroscopy of the plasma often did change as a function of interrogation position.
[0600] For example,
[0601] Table 2d shows specifically each of the spectral lines identified in the adjustable plasma 4 when a gold electrode 1 was utilized to create the plasma 4.
TABLE-US-00012 TABLE 2d λ meas. − λ tab. λ meas. λ tab. En Em Amn Transition (nm) (nm) (nm) (1/cm) (1/cm) gn gm (1/s) NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (1-0) 214.7 214.7000 0.0000 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (0-0) 226.9 226.8300 −0.0700 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (0-1) 236.3 236.2100 −0.0900 Au | 5d.sup.106s .sup.2S.sub.1/2 − 5d.sup.106p .sup.2P.sup.0.sub.3/2 242.795 242.7900 −0.0050 0 41174.613 2 4 1.99E+8 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (0-2) 247.1 246.9300 −0.1700 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (0-3) 258.3 258.5300 0.2300 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (1-1) 267.1 267.0600 −0.0400 Au | 5d.sup.106s .sup.2S.sub.1/2 − 5d.sup.106p .sup.2P.sup.0.sub.1/2 267.595 267.59 −0.0050 0 37358.991 2 2 1.64E+8 NO A.sup.2Σ.sup.+ − X.sup.2Π γ-system: (0-4) 271 271.1400 0.1400 Au | 5d.sup.96s.sup.2 .sup.2D.sub.5/2 − 5d.sup.9(.sup.2D.sub.5/2)6s6p .sup.24.sup.0.sub.7/2 274.825 274.82 −0.0050 9161.177 45537.195 6 8 OH A.sup.2Σ − X.sup.2Π (1-0) 281.2 281.2000 0.0000 OH A.sup.2Σ − X.sup.2Π (1-0) 282 281.9600 −0.0400 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (4-2) 295.32 295.3300 0.0100 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (3-1) 296.2 296.1900 −0.0100 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (2-0) 297.7 297.7000 0.0000 OH A.sup.2Σ − X.sup.2Π: (0-0) 306.537 306.4600 −0.0770 OH A.sup.2Σ − X.sup.2Π: (0-0) 306.776 306.8400 0.0640 OH A.sup.2Σ − X.sup.2Π: (0-0) 307.844 307.8700 0.0260 OH A.sup.2Σ − X.sup.2Π: (0-0) 308.986 309.0700 0.0840 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (2-1) 313.57 313.5800 0.0100 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (1-0) 316 315.9200 −0.0800 O.sub.2 (B.sup.3Σ.sup.−.sub.u − X.sup.3Σ.sup.−.sub.g) (0-14) 337 337.0800 0.0800 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (0-0) 337.1 337.1400 0.0400 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (2-3) 350.05 349.9700 −0.0800 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (1-2) 353.67 353.6400 −0.0300 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (0-1) 357.69 357.6500 −0.0400 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (1-0) 358.2 358.2000 0.0000 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (2-4) 371 370.9500 −0.0500 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (1-3) 375.54 375.4500 −0.0900 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (0-2) 380.49 380.4000 −0.0900 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (1-1) 388.4 388.4200 0.0200 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (0-0) 391.4 391.3700 −0.0300 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (1-4) 399.8 399.7100 −0.0900 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (0-3) 405.94 405.8100 −0.1300 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (4-8) 409.48 409.4900 0.0100 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (2-3) 419.96 420.0000 0.0400 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (1-2) 423.65 423.6400 −0.0100 N.sub.2.sup.+ (B.sup.2Σ.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (0-1) 427.785 427.7700 −0.0150 N.sub.2 (C.sup.3Π.sub.u − B.sup.3Π.sub.g) 2.sup.+-system (3-8) 441.67 441.6200 −0.0500 Au | 5d.sup.9(.sup.2D.sub.5/2)6s6p .sup.24.sup.0.sub.7/2 − 5d.sup.9(.sup.2D.sub.5/2)6s6p 10.sub.7/2 448.8263 448.7500 −0.0763 45537.195 67811.329 8 8 N.sub.2.sup.+ (B.sup.2Π.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (1-3) 465.1 465.1300 0.0300 N.sub.2.sup.+ (B.sup.2Π.sup.+.sub.u − X.sup.2+.sub.g) 1.sup.−-system (0-2) 470.9 470.8400 −0.0600 Na | 3s .sup.2S.sub.1/2 − 3p .sup.2P.sup.0.sub.3/2 588.99 588.995 0.0050 H | 2p .sup.2P.sub.3/2 − 3d .sup.2D.sub.5/2 656.2852 655.8447 −0.4405 82259.287 97492.357 4 6 6.47E+7 N | 3s .sup.4P.sub.5/2 − 3p .sup.4S.sub.3/2 746.8312 746.8815 0.0503 83364.62 96750.84 6 4 1.93E+7 N.sub.2 (B.sup.3Π.sub.g − A.sup.3Σ.sup.−.sub.u) 1.sup.+ -system 750 749.9618 −0.0382 O | 3s .sup.5S.sub.2 − 3p.sup.5P.sub.3 777.1944 776.8659 −0.3285 73768.2 86631.454 5 7 3.69E+7 O | 3s .sup.3S.sub.1 − 3p .sup.3P.sub.2 844.6359 844.2905 −0.3454 76794.978 88631.146 3 5 3.22E+7 N | 3s .sup.4P.sub.5/2 − 3p .sup.4D.sub.7/2 868.0282 868.2219 0.1937 83364.62 94881.82 6 8 2.46E+7 O | 3p .sup.5P.sub.3 − 3d .sup.5D.sub.4 926.6006 926.3226 −0.2780 86631.454 97420.63 7 9 4.45E+7
[0602] A variety of species associated with the gold metallic electrode 1 are identified in Table 2d. These species include, for example, gold from the electrodes 1, as well as common species including, NO, OH, N2, etc. It is interesting to note that some species' existence and/or intensity (e.g., amount) is a function of location within the adjustable plasma. Accordingly, this suggests that various species can be caused to occur as a function of a variety of processing conditions (e.g., power, location, composition of electrode 1, etc.) of the invention.
Examples 8-10
Manufacturing Gold-Based Nanocrystal Suspensions GB-018, GB-019 and GB-020
[0603] In general, each of Examples 8-10 utilize certain embodiments of the invention associated with the apparatuses generally shown in
[0604] Purified water (discussed elsewhere herein) was mixed with NaHCO.sub.3 in a range of about 0.396 to 0.528 g/L of NaHCO.sub.3 and was used as the liquid 3 input into trough member 30a. While this range of NaHCO.sub.3 utilized was effective, it should not be viewed as limiting the metes and bounds of the invention. The depth “d” (refer to
[0605] The rate of flow of the water 3 into the trough member 30a ranged from about 150 ml/minute to at least 280 ml/minute. Such flow of water 3 was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 150 milliliters per minute. Tygon® tubing having a diameter of ¼″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30a by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30a as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30a such that when the reservoir overflowed, a relatively steady flow of water 3 into the end 31 of the V-shaped trough member 30a occurred.
[0606] There were 5 electrode sets used in Examples 8-10 and one electrode set was a single electrode set 1a/5a located in the trough member 30a. The plasma 4 from electrode 1a in trough member 30a was created with an electrode 1 similar in shape to that shown in
[0607] The output of the processing-enhanced, conditioned water 3′ was collected into a reservoir 41 and subsequently pumped by another pump 40′ into a second trough member 30b, at substantially the same rate as pump 40 (e.g., there was minimal evaporation in trough member 30a). The second trough member 30b shown in
[0608] With regard to
[0609] Each of Tables 3a-3c contains processing information relative to each of the 4 electrode sets by “Set #”. Each electrode of the 4 electrode sets in trough 30b was set to operate at a specific target voltage. Actual operating voltages of about 255 volts, as listed in each of Tables 3a-3c, were applied to the four electrode sets. The distance “c-c” (with reference to
[0610] The water 3 used in Examples 8-10 was produced by a Reverse Osmosis process and deionization process and was mixed with the NaHCO.sub.3 processing-enhancer and together was input into the trough member 30a. In essence, Reverse Osmosis (RO) is a pressure driven membrane separation process that separates species that are dissolved and/or suspended substances from the ground water. It is called “reverse” osmosis because pressure is applied to reverse the natural flow of osmosis (which seeks to balance the concentration of materials on both sides of the membrane). The applied pressure forces the water through the membrane leaving the contaminants on one side of the membrane and the purified water on the other. The reverse osmosis membrane utilized several thin layers or sheets of film that are bonded together and rolled in a spiral configuration around a plastic tube. (This is also known as a thin film composite or TFC membrane.) In addition to the removal of dissolved species, the RO membrane also separates out suspended materials including microorganisms that may be present in the water. After RO processing a mixed bed deionization filter was used. The total dissolved solvents (“TDS”) after both treatments was about 0.2 ppm, as measured by an Accumet® AR20 pH/conductivity meter.
TABLE-US-00013 TABLE 3a 0.528 mg/ml of NaHCO.sub.3 (Au) Run ID: GB-018 Flow Rate: 280 ml/min Voltage: 255 V NaHCO.sub.3: 0.528 mg/ml Wire Dia.: .5 mm Configuration: J/J PPM: 2.9 Zeta: −98.84 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 3.5/88.9 3 5c N/A 255 Tapered .sup. 5c′ N/A 3″Deep 3.5/88.9 4 5d N/A 255 .sup. 5d′ N/A 3.5/88.9 5 5e N/A 255 .sup. 5e′ N/A 376.2** Output Water Temperature 80 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
TABLE-US-00014 TABLE 3b 0.396 mg/ml of NaHCO.sub.3 (Au) Run ID: GB-019 Flow Rate: 150 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: 1 mm Configuration: J/J PPM: 23.6 Zeta: −56.6 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25/6.35 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 3.5/88.9 3 5c N/A 255 Tapered .sup. 5c′ N/A 3″Deep 3.5/88.9 4 5d N/A 255 .sup. 5d′ N/A 3.5/88.9 5 5e N/A 255 .sup. 5e′ N/A 376.2** Output Water Temperature 97 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
TABLE-US-00015 TABLE 3c 0.396 mg/ml of NaHCO.sub.3 (Au) Run ID: GB-020 Flow Rate: 250 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: 1 mm Configuration: J/J PPM: 4.9 Zeta: −58.01 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 3.5/88.9 3 5c N/A 255 Tapered .sup. 5c′ N/A 3″Deep 3.5/88.9 4 5d N/A 255 .sup. 5d′ N/A 3.5/88.9 5 5e N/A 255 .sup. 5e′ N/A 376.2** Output Water Temperature 86 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
[0611]
[0612]
[0613]
[0614] It should be noted that the dynamic light scattering particle size information is different from the TEM measured histograms because dynamic light scattering uses algorithms that assume the crystals are all spheres (which they are not) as well as measures the hydrodynamic radius (e.g., the crystal's influence on the water is also detected and reported in addition to the actual physical radii of the crystals). Accordingly, it is not surprising that there is a difference in the reported crystal sizes between those reported in the TEM histogram data and those reported in the dynamic light scattering data, just as in the other Examples included herein.
Example 11
Manufacturing Gold-Based Nanoparticles/Nanoparticle Solutions or Colloids IAC-202-7 by a Batch Process
[0615] This Example utilizes a batch process according to the present invention.
[0616] Table 4a shows a matrix where the amount of processing enhancer baking soda (i.e., NaHCO.sub.3) varies from about 1 gram/gallon to about 2 grams/gallon (i.e., about 0.264 g/L to about 0.528 g/L); and the dwell time reflected in Table 4a in the apparatus of
[0617] Accordingly, Table 4a shows that a number of variables (e.g., processing enhancer and predetermined dwell time) influence both the amount or concentration of gold nanocrystals in water, and the size distribution of the gold nanocrystals. In general, as the concentration of the processing enhancer increases from about 1 g/gallon (0.264 g/L) to about 2 g/gallon (0.528 g/L), the concentration (i.e., “ppm”) more or less increases under a given set of processing conditions. However, in some cases the particle size distribution (“psd”) unfavorably increases such that the formed nanocrystals were no longer stable, and they “settled”, as a function of time (e.g., an unstable suspension was made). These settling conditions were not immediate thus suggesting that this suspension of nanocrystals in water could be processed immediately into a useful product, such as, for example, a gel or cream. This Example shows clearly various important effects of multiple processing variables which can be translated, at least directionally, to the inventive continuous processes disclosed elsewhere herein. These data are illustrative and should not be viewed as limiting the metes and bounds of the present invention. Moreover, these illustrative data should provide an artisan of ordinary skill with excellent operational directions to pursue.
[0618] As a specific example, Table 4c shows that a first electrode Set #1 (i.e.,
TABLE-US-00016 TABLE 4a Pretreatment Dwell (minutes) 20 40 60 1AC-201 1AC-202 1AC-201 1AC-202 1AC-201 1AC-202 NaHCO.sub.3 .264 ppm 1AC- 11.8 1AC- 11.1 1AC- 13.5 1AC- 11.4 1AC- 14.3 1AC- 12.2 (mg/ml) psd 201-9 18.4 202-1 19.1 201-8 19.5 202-2 18.4 201-7 16.8 202-3 19.6 .396 ppm 1AC- 20.1 1AC- 16.1 1AC- 21.4 1AC- settled 1AC- 23.3 1AC- settled psd 201-6 21.4 202-7 32.3 201-5 126 202-8 84.8 201-4 36.3 202-9 23.8 .528 ppm 1AC- 27.4 1AC- 23 1AC- 31.1 1AC- 24.9 1AC- settled 1AC- settled psd 201-1 17.1 202-4 43.8 201-2 21.6 202-5 21.4 201-3 190 202-6 settled
TABLE-US-00017 TABLE 4b Pretreatment Dwell (minutes) Current 20 40 60 Amps 1AC-201 1AC-202 1AC-201 1AC-202 1AC-201 1AC-202 NaHCO.sub.3 .264 min 1AC- 0.405 1AC- 0.382 1AC- 0.41 1AC- 0.411 1AC- 0.432 1AC- 0.461 (mg/ml) max 201-9 1.1 202-1 1 201-8 1 202-2 1.06 201-7 1 202-3 1.13 .396 min 1AC- 0.554 1AC- 0.548 1AC- 0.591 1AC- 0.598 1AC- 0.617 1AC- 0.681 max 201-6 1.6 202-7 1.35 201-5 1.6 202-8 1.43 201-4 1.6 202-9 1.43 .528 min 1AC- 0.686 1AC- 0.735 1AC- 0.843 1AC- 0.769 1AC- 0.799 1AC- 0.865 max 201-1 1.82 202-4 1.6 201-2 2.06 202-5 2 201-3 2.01 202-6 2.1
TABLE-US-00018 TABLE 4c 1.5 g/Gal of NaHCO.sub.3 (Au) Run ID: 1AC-202-7 Pretreatment: 20 min GZA in 3600 ml Volume: 800 ml Run time: 35 minutes Voltage: 250 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: .5 mm Configuration: J/J PPM: 16.1 Zeta: n/a Distance “x” Set# Electrode# in/mm Voltage 1 1a 0.25/6.35 750 5a N/A 750 2 5b N/A 250 .sup. 5b′ N/A
[0619]
[0620]
[0621]
[0622] It should be noted that the dynamic light scattering particle size information is different from the TEM measured histograms because dynamic light scattering uses algorithms that assume the nanocrystals are all spheres (which they are not) as well as measures the hydrodynamic radius (e.g., the nanocrystal's influence on the water is also detected and reported in addition to the actual physical radii of the nanocrystals). Accordingly, it is not surprising that there is a difference in the reported nanocrystals sizes between those reported in the TEM histogram data and those reported in the dynamic light scattering data, just as in the other Examples included herein.
Example 12
Manufacturing Gold-Based Nanoparticles/Nanoparticle Solutions or Colloids IAC-261 by a Batch Process
[0623] This Example utilizes a batch process according to the present invention.
[0624] The amount of processing enhancer baking soda (i.e., NaHCO.sub.3) was about 1.5 grams/gallon (i.e., about 0.396 g/L). The amount of time that the water 3 with processing enhancer was exposed to the plasma 4 was about 60 minutes, prior to subsequent processing in the apparatus shown in
[0625] The applied voltage for each plasma 4 made by electrode 1 was about 750 volts. This voltage was achieved by a transformer 60 (i.e., the Balanced Mid-Point Referenced Design) discussed elsewhere herein.
[0626] A second and different transformer was electrically connected to the electrodes 5a/5b shown in
[0627] The amount of gold nanoparticles produced in the suspension was about 13.7 ppm as measured by the atomic absorption spectroscopy techniques discussed elsewhere herein. The sizes and shapes of the nanoparticles made according to this Example are fully discussed in Table 12 herein
[0628]
[0629]
Example 13
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspensions GB-154-20 Hz, GB-157-40 Hz, GB-159-60 Hz, GB-161-80 Hz, GB-173-100 Hz and GB-156-300 Hz)
[0630] In general, this Example used the same manufacturing set-up used for making GB-134 in Example 16, and for the sake of brevity, the specifics of the trough apparatus used are discussed in detail in that Example. The primary difference in making the suspensions or colloids in this Example is that different sine waveform frequencies from a programmable AC source were used as electrical inputs to the electrodes 5a/5b.
[0631] In particular, sine wave AC frequencies as low as 20 Hz and as high as 300 Hz were utilized to make nanocrystal suspensions or colloids, in accordance with the teachings herein. The AC power source 501AC utilized a Chroma 61604 programmable AC source. The applied voltage was 300 volts. The waveform was a sine wave at six different frequencies-20, 40, 60, 80, 100 and 300 Hz. The applied current varied between 4.2 amps and 4.8 amps.
[0632]
[0633]
[0634]
[0635]
[0636]
[0637]
[0638] It is clear form this Example that particle size “mode” and particle size distribution both increased as a function of increasing the frequency AC sine waveform under the conditions of this Example.
Example 14
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspensions (GB-166-Sine, GB-165-Square and GB-162-Triangle)
[0639] In general, this Example used the same manufacturing set-up used for making GB-134 in Example 16, and for the sake of brevity, the specifics of the trough apparatus used are discussed in detail in that Example. The primary difference in making the suspensions or colloids in this Example was three different types of waveforms (i.e., sine, square, and triangular waves) were generated by a BK Precision 4040 20 MHz function generator, 501FG. The waveform output was input into a chroma 61604 programmable AC source, 501AC. The applied voltage for the sine waves (“SI”) and square waves (“SQ”) was 300 volts, while the applied voltage for the triangular-shaped waveforms (“TR”) was 250 volts. Each of these waveforms is shown in
[0640]
[0641]
[0642]
Example 15
Manufacturing Gold-Based Nanoparticles/Nanoparticle Suspensions (GB-163 and GB-164)
[0643] In general, this Example used the same manufacturing set-up used for making GB-134 in Example 16, and for the sake of brevity, the specifics of the trough apparatus used are discussed in detail in that Example. The primary difference in making the suspensions or colloids in this Example was that two different duty cycles for the triangular waveforms from the signal wave generator 501FG and programmable AC power source 501AC (i.e., discusses in Example 14) were used. The applied voltage for each triangular waveform was 250 volts. Specifically, each of GB-166 and GB-164 utilized the triangular-shaped waveforms TR-1, TR-2 and TR-3 shown in
[0644]
[0645]
Example 16
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspensions (GB-134); (GB-098, GB-113 and GB-118); (GB-120 and GB-123); (GB-139); (GB-141 and GB-144); (GB-079, GB-089 and GB-062); and (GB-076 and GB-077)
[0646] In general, this Example 16 utilizes certain embodiments of the invention associated with the apparatuses generally shown in
TABLE-US-00019 TABLE 5 Run ID: GB-134 GB-098 GB-113 GB-118 GB-120 GB-123 GB-139 Flow In (ml/min) 150 150 150 150 150 150 150 Rate: Out (ml/min) 110 110 110 110 110 110 110 Set # 1 750 750 750 750 750 750 750 Volts: Set # 2 300 297 300 300 300 300 300 Set #'s 3-9 300 297 300 300 300 300 300 PE: NaHCO3 (mg/ml) 0.53 0.40 0.53 0.53 0.53 0.53 0.53 Wire Diameter (mm) 1.0 1.0 1.0 1.0 1.0 1.0 1.0 Contact “W.sub.L” (in/mm) .75/19 1/25 0.5/13 0.5/13 0.5/13 0.5/13 0.75/19 Electrode Config. FIG. 17b 17b 17b 17c 17b 17b 17d Produced Au PPM 8.9 8.0 10.3 9.3 10.4 10.1 10.0 Output Temp ° C. at 32 85 93 88 86 84 93 87 Dimensions Plasma 4 FIGS. 18a 18a 18a 18a 18a 18a 18a Process FIGS. 20h, 21e 20f, 21b 20f, 21b 20f, 21b 20g, 21d 20g, 21d 20c, 20h 21e, 21f, 21g M1 (in/mm) 2/51 1/25 2/51 2/51 3.5/89 2/51 2/51 M2 (in/mm) n/a n/a n/a n/a n/a n/a n/a L.sub.T (in/mm) 36/914 48/1219 36/914 36/914 36/914 36/914 36/914 d (in/mm) .75/19 1/25 0.5/13 0.5/13 0.5/13 0.5/13 0.75/19 S (in/mm) 1.5/38.1 3/76.2 2.5/63.5 2.5/63.5 2.5/63.5 2.5/63.5 1.5/38.1 Electrode Curr. (A) 0.56 0.53 0.53 0.52 0.51 0.48 FIG. 54d Total Curr. Draw (A) n/a n/a n/a n/a n/a n/a n/a Hydrodynamic r (nm) 16.2 20.02 12.8 12.3 12.8 12.8 15.9 TEM Avg. Dia. (nm) 17.48 20.03 13.02 12.06 13.34 13.65 13.97 “c-c” (mm) 76 83 83 83 83 83 83 Set electrode # 1a 1a 1a 1a 1a 1a 1a 1 “x” (in/mm) 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 electrode # 5a 5a 5a 5a 5a 5a 5a “c-c” (mm) 89 83 89 89 89 89 83 Set electrode # 5b 5b 5b 5b 5b 5b 5b 2 “x” (in/mm) n/a n/a n/a n/a n/a n/a n/a electrode # .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ “c-c” (mm) 38 76 59 56 57 38 76 Set electrode # 5c 5c 5c 5c 5c 5c 5c 3 electrode # .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ “c-c” (mm) 38 105 60 59 64 38 76 Set electrode # 5d 5d 5d 5d 5d 5d 5d 4 electrode # .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ “c-c” (mm) 89 143 70 68 70 44 127 Set electrode # 5e 5e 5e 5e 5e 5e 5e 5 electrode # .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ “c-c” (mm) 89 165 84 103 70 51 127 Set electrode # 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 6 electrode # 5f′ 5f′ 5f′ 5f′ 5f′ 5f′ 5f′ “c-c” (mm) 89 178 108 102 64 54 127 Set electrode # 5g 5g 5g 5g 5g 5g 5g 7 electrode # .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ “c-c” (mm) 178 178 100 100 76 54 216 Set electrode # 5h 5h 5h 5h 5h 5h 5h 8 electrode # .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ “c-c” (mm) 89 216 127 135 76 57 83 Set electrode # n/a 5i.sup. 5i.sup. 5i.sup. 5i.sup. 5i.sup. n/a 9 electrode # n/a 5i′ 5i′ 5i′ 5i′ 5i′ n/a “c-c” (mm) n/a 76 191 178 324 464 n/a Run ID: GB-141 GB-144 GB-079 GB-089 GB-062 GB-076 GB-077 Flow In (ml/min) 150 110 150 150 150 150 150 Rate: Out (ml/min) 110 62 110 110 110 110 110 Set # 1 750 750 750 750 750 750 750 Volts: Set # 2 299 299 255 255 750 750 750 Set #'s 3-9 299 299 255 255 249 306 313 PE: NaHCO3 (mg/ml) 0.53 0.53 0.40 0.40 0.40 0.53 0.40 Wire Diameter (mm) 1.0 1.0 0.5 0.5 0.5 0.5 0.5 Contact “W.sub.L” (in/mm) 0.5/13 0.5/13 2/51 2/51 2/51 1/25 1/25 Electrode Config. FIG. 17d 17d 17b 17b 17b 17b 17b Produced Au PPM 10.1 20.2 10.8 12.4 16.7 7.8 7.5 Output Temp ° C. at 32 86 89 94 99 95 98 97 Dimensions Plasma 4 FIGS. 18a 18a 18a 18a 18b 18b 18b Process FIGS. 20c, 20h 20c, 20h 20d, 21c 20d, 21c 20e, 21c 20e, 22b 20e, 22b 21e, 21f, 21e, 21f, 21g 21g M1 (in/mm) 2/51 2/51 1/25 0.75/19 1/25 2.7/68.6 2.7/686 M2 (in/mm) n/a n/a n/a n/a n/a 0.5/13 0.5/13 L.sub.T (in/mm) 36/914 36/914 24/610 24/610 24/610 24/610 24/610 d (in/mm) 0.5/13 0.5/13 2/51 2/51 2/51 1/25 1/25 S (in/mm) 1.5/38.1 1.5/38.1 3.3/83.8 3.3/83.8 3.3/83.8 3.5/88.9 3.5/88.9 Electrode Curr. (A) FIG. 55d FIG. 56d 0.66 n/a 0.7 0.51 0.48 Total Curr. Draw (A) n/a n/a 11.94 8.98 12.48 13.62 12.47 Hydrodynamic r (nm) 26.2 16.4 14.9 17.2 17.0 9.7 11.5 TEM Avg. Dia. (nm) 11.42 18.12 10.63 15.89 11.75 11.07 8.69 “c-c” (mm) n/a 83 n/m n/m n/m n/m n/m Set electrode # n/a 1a 1a 1a 1a 1a 1a 1 “x” (in/mm) n/a 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 electrode # n/a 5a 5a 5a 5a 5a 5a “c-c” (mm) 83 83 n/m n/m n/m n/m n/m Set electrode # 5b 5b 5b 5b 1b 1b 1b 2 “x” (in/mm) n/a n/a n/a n/a 0.25/6.4 0.25/6.4 0.25/6.4 electrode # .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ 5b 5b 5b “c-c” (mm) 76 76 n/m n/m n/m n/m n/m Set electrode # 5c 5c 5c 5c 5c 5c 5c 3 electrode # .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ “c-c” (mm) 76 76 n/m n/m n/m n/m n/m Set electrode # 5d 5d 5d 5d 5d 5d 5d 4 electrode # .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ “c-c” (mm) 127 127 n/m n/m n/m n/m n/m Set electrode # 5e 5e 5e 5e 5e 5e 5e 5 electrode # .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ “c-c” (mm) 127 127 n/m n/m n/m n/m n/m Set electrode # 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 6 electrode # 5f′ 5f′ 5f′ 5f′ 5f′ 5f′ 5f′ “c-c” (mm) 127 127 n/m n/m n/m n/m n/m Set electrode # 5g 5g 5g 5g 5g 5g 5g 7 electrode # .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ “c-c” (mm) 216 216 n/m n/m n/m n/m n/m Set electrode # 5h 5h 5h 5h 5h 5h 5h 8 electrode # .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ “c-c” (mm) 83 83 n/m n/m n/m n/m n/m Set electrode # n/a n/a n/a n/a 5i.sup. 5i.sup. 5i.sup. 9 electrode # n/a n/a n/a n/a 5i′ 5i′ 5i′ “c-c” (mm) n/a n/a n/a n/a n/m n/m n/m
[0647] All trough members 30a′ and 30b′ in the aforementioned Figures were made from 1/8″ (about 3 mm) thick plexiglass, and ¼″ (about 6 mm) thick polycarbonate, respectively. The support structure 34 (not shown in many of the Figures but discussed elsewhere herein) was also made from plexiglass which was about ¼″ thick (about 6-7 mm thick). In contrast to the embodiments shown in
[0648] Table 5 shows that the processing enhancer NaHCO.sub.3 was added to purified water (discussed elsewhere herein) in amounts of either about 0.4 mg/ml or 0.53 mg/ml. It should be understood that other amounts of this processing enhancer also function within the metes and bounds of the invention. The purified water/NaHCO.sub.3 mixture was used as the liquid 3 input into trough member 30a′. The depth “d” of the liquid 3′ in the trough member 30a′ (i.e., where the plasma(s) 4 is/are formed) was about 7/16″ to about ½″ (about 11 mm to about 13 mm) at various points along the trough member 30a′. The depth “d′” was partially controlled through use of the dam 80 (shown in
[0649] The rate of flow of the liquid 3′ into the trough member 30a′ as well as into trough member 30b′, was about 150 ml/minute for all but one of the formed samples (i.e., GB-144 which was about 110 ml/minute) and the rate of flow out of the trough member 30b′ at the point 32 was about 110 ml/minute (i.e., due to evaporation) for all samples except GB-144, which was about 62 ml/minute. The amount of evaporation that occurred in GB-144 was a greater percent than the other samples because the dwell time of the liquid 3″ in the trough member 30b′ was longer relative to the other samples made according to this embodiment. Other acceptable flow rates should be considered to be within the metes and bounds of the invention.
[0650] Such flow of liquid 3′ was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 150 milliliters per minute for all samples except GB-144 which was, for example, 110 ml/minute. Tygon® tubing having a diameter of ¼″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30′a by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30a′ as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30a′ such that when the reservoir overflowed, a relatively steady flow of liquid 3′ into the end 31 of the V-shaped trough member 30a′ occurred.
[0651] Table 5 shows that there was a single electrode set 1a/5a, or two electrode sets 1a/5a, utilized in this Example 18. The plasma(s) 4 was/were created with an electrode 1 similar in shape to that shown in
[0652] As shown in
[0653] With regard to
[0654] Table 5 refers to each of the electrode sets by “Set #” (e.g., “Set 1” through “Set 9”). Each electrode of the 1/5 or 5/5 electrode sets was set to operate within a specific voltage range. The voltages listed in Table 5 are the voltages used for each electrode set. The distance “c-c” (with reference to
[0655] All materials for the electrodes 1/5 were obtained from ESPI, having an address of 1050 Benson Way, Ashland, Oreg. 97520. All materials for the electrodes 5/5 in runs GB-139, GB-141, GB-144, GB-076, GB-077, GB-079, GB-089, GB-098, GB-113, GB-118, GB-120 and GB-123 were obtained from Alfa Aesar, having an address of 26 Parkridge Road, Ward Hill, Mass. 01835. All materials for the electrodes 5/5 in run GB-062 were obtained from ESPI, 1050 Benson Way, Ashland, Oreg. 97520.
[0656]
[0657]
[0658]
[0659] Reference is now made to
[0660] With reference to
[0661] The movement of the electrodes 5 into the female receiver tubes o5 can occur by monitoring a variety of specific process parameters which change as a function of time (e.g., current, amps, nanocrystals concentration, optical density or color, conductivity, pH, etc.) or can be moved a predetermined amount at various time intervals to result in a fixed movement rate, whichever may be more convenient under the totality of the processing circumstances. In this regard,
[0662] Energy absorption spectra were obtained for the samples in Example 16 by using UV-VIS spectroscopy. This information was acquired using a dual beam scanning monochromator system capable of scanning the wavelength range of 190 nm to 1100 nm. The Jasco V-530 UV-Vis spectrometer was used to collect absorption spectroscopy. Instrumentation was setup to support measurement of low-concentration liquid samples using one of a number of fused-quartz sample holders or “cuvettes”. The various cuvettes allow data to be collected at 10 mm, Imm or 0.1 mm optic path of sample. Data was acquired over the wavelength range using between 250-900 nm detector with the following parameters; bandwidth of 2 nm, with data pitch of 0.5 nm, a silicon photodiode with a water baseline background. Both deuterium (D2) and halogen (WI) scan speed of 400 nm/mm sources were used as the primary energy sources. Optical paths of these spectrometers were setup to allow the energy beam to pass through the center of the sample cuvette. Sample preparation was limited to filling and capping the cuvettes and then physically placing the samples into the cuvette holder, within the fully enclosed sample compartment. Optical absorption of energy by the materials of interest was determined. Data output was measured and displayed as Absorbance Units (per Beer-Lambert's Law) versus wavelength.
[0663] Spectral patterns in a UV-Visible range were obtained for each of the solutions/colloids produced in Example 16.
[0664] Specifically,
[0665]
[0666] In general, UV-Vis spectroscopy is the measurement of the wavelength and intensity of absorption of near-ultraviolet and visible light by a sample. Ultraviolet and visible light are energetic enough to promote outer electrons to higher energy levels. UV-Vis spectroscopy can be applied to molecules and inorganic ions or complexes in solution or suspension.
[0667] The UV-Vis spectra have broad features that can be used for sample identification but are also useful for quantitative measurements. The concentration of an analyte in solution can be determined by measuring the absorbance at some wavelength and applying the Beer-Lambert Law.
Example 17
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspension GB-056
[0668] In general, Example 17 utilizes certain embodiments of the invention associated with the apparatuses generally shown in
[0669] Purified water (discussed elsewhere herein) was mixed with about 0.396 g/L of NaHCO.sub.3 and was used as the liquid 3 input into trough member 30a′. The depth “d” (refer to
[0670] The rate of flow of the liquid 3′ into the trough member 30a′ was about 150 ml/minute and the rate of flow out of the trough member 30b′ at the point 32 was about 110 ml/minute (i.e., due to evaporation). Such flow of liquid 3′ was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 150 milliliters per minute. Tygon® tubing having a diameter of ¼″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30′a by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30a′ as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30a′ such that when the reservoir overflowed, a relatively steady flow of liquid 3′ into the end 31 of the V-shaped trough member 30a′ occurred.
[0671] There was a single electrode set 1a/5a utilized in this Example 17. The plasma 4 was created with an electrode 1 similar in shape to that shown in
[0672] As shown in
[0673] With regard to
[0674] Table 6 refers to each of the 4 electrode sets by “Set #”. Each electrode of the 4 electrode sets was set to operate within a specific voltage range. The actual voltages, listed in Table 10, were about 255 volts. The distance “c-c” (with reference to
[0675] All materials for the electrodes 1/5 were obtained from ESPI having an address of 1050 Benson Way, Ashland, Oreg. 97520.
TABLE-US-00020 TABLE 6 0.396 mg/ml of NaHCO.sub.3 (Au) Run ID: GB-056 Flow Rate: 150 ml/min Voltage: 255 V NaHCO.sub.3: 0.396 mg/ml Wire Dia.: .5 mm Configuration: J/J PPM: 12 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25/6.35 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 3.5/88.9 3 5c N/A 255 Tapered .sup. 5c′ N/A 3″Deep 3.5/88.9 4 5d N/A 255 .sup. 5d′ N/A 3.5/88.9 5 5e N/A 255 .sup. 5e′ N/A 376.2** Output Water Temperature 98 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water outlet
[0676]
[0677]
[0678]
[0679]
[0680] Likewise,
[0681] While
[0682] Taken together, these data suggest that exposure of the inventive compositions disclosed herein to certain constituents in, for example, mouse saliva, can cause a clustering or clumping together of the nanocrystals suspended in the liquid. Accordingly, prolonged exposure to certain proteins may have a “denaturing” effect on these inventive compositions. This “denaturing” effect is manageable, and without wishing to be bound by any particular theory or explanation, may be very desirable in that such reactivity due to very “clean” surfaces may support desirable in vivo activity (e.g., certain protein-binding mechanisms).
Example 18
Manufacturing Gold-Based Nanocrystals/Nanocrystal Suspensions (GB-151, GB-188, GB-175, GB-177, GB-176, GB-189, GB-194, GB-195, GB-196, GB-198 and GB-199)
[0683] In general, this Example utilizes certain embodiments of the invention associated with the apparatuses generally shown in
TABLE-US-00021 TABLE 7 Run ID: GB-151 GB-188 GB-175 GB-177 GB-176 Flow In (ml/min) 220 230 230 230 230 Rate: Out (ml/min) 175 184 184 184 184 Volts: Set # 1 750 750 750 750 n/a Set #'s 2-8 230 198 210 208 210 PE: NaHCO3 (mg/ml) 0.53 0.53 0.53 0.53 0.53 Wire Diameter (mm) 1.0 1.0 2.0 1.1 3.0 Contact “W.sub.L” (in/mm) 1/25 1/25 1/25 1/25 1/25 Electrode Separation “y” (in/mm) .25/6.4 .25/6.4 .25/6.4 .25/6.4 .25/6.4 Electrode Config. FIG. 17b 17b 17b 17b 17b Produced Au PPM 8.3 8.4 10.5 9.5 10.1 Output Temp ° C. at 32 89 84 89 88 86 Dimensions Plasma 4 FIGS. 18a 18a 18a 18a n/a Process FIGS. 21d 21d 21d 21d 21d M1 (in/mm) 2/51 1.5/38 1.5/38 1.5/38 1.5/38 L.sub.T (in/mm) 30/762 36/914 36/914 36/914 36/914 d (in/mm) 1/25 1/25 1/25 1/25 1/25 S (in/mm) 1.5/38 1.5/38 2/51 2/51 2/51 Electrode Curr. (A) 0.89 .85 .93 .80 .88 Total Curr. Draw (A) n/m 6.06 7.02 6.84 6.82 Hydrodynamic r (nm) 11.6 12 14 13.1 13.2 TEM Avg. Dia. (nm) 10.85 10.63 11.76 10.85 10.42 “c-c” (mm) 152 76 76 76 n/a Set electrode # 1a 1a 1a 1a n/a 1 “x” (in/mm) 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 n/a electrode # 5a 5a 5a 5a n/a “c-c” (mm) 63 102 102 102 102 Set electrode # 5b 5b 5b 5b 5b 2 “x” (in/mm) n/a n/a n/a n/a n/a electrode # .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ “c-c” (mm) 76 76 76 76 76 Set electrode # 5c 5c 5c 5c 5c 3 electrode # .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ “c-c” (mm) 76 76 76 76 76 Set electrode # 5d 5d 5d 5d 5d 4 electrode # .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ “c-c” (mm) 114 127 127 127 127 Set electrode # 5e 5e 5e 5e 5e 5 electrode # .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ “c-c” (mm) 114 127 127 127 127 Set electrode # 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 6 electrode # 5f′ 5f′ 5f′ 5f′ 5f′ “c-c” (mm) 114 152 152 152 152 Set electrode # 5g 5g 5g 5g 5g 7 electrode # .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ “c-c” (mm) 127 178 178 178 178 Set electrode # 5h 5h 5h 5h 5h 8 electrode # .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ “c-c” (mm) 76 76 76 76 76 Run ID: GB-189 GB-194 GB-195 GB-196 GB-198 GB-199 Flow In (ml/min) 230 250 250 250 150 150 Rate: Out (ml/min) 184 200 200 200 120 120 Volts: Set # 1 750 750 750 750 n/a 750 Set #'s 2-8 208 210 210 210 205 205 PE: NaHCO3 (mg/ml) 0.53 0.53 0.53 0.53 0.26 0.26 Wire Diameter (mm) 1.2 4.0 1.3 5.0 1.4 6.0 Contact “W.sub.L” (in/mm) 1/25 1/25 1/25 1/25 1/25 1/25 Electrode Separation “y” (in/mm) .25/6.4 .25/6.4 .25/6.4 .25/6.4 .125/3.18 .125/3.18 Electrode Config. FIG. 17b 17b 17b 17b 17b 17b Produced Au PPM 8.4 8.7 7.7 8.7 9.9 12.4 Output Temp ° C. at 32 85 93 96 89 74 80 Dimensions Plasma 4 FIGS. 18a 18a 18a 18a n/a 18a Process FIGS. 21d 21d 21d 21d 21d 21d M1 (in/mm) 1.5/38 .75/19 .5/13 1/25 1.5/38 1.5/38 L.sub.T (in/mm) 36/914 36/914 36/914 36/914 36/914 36/914 d (in/mm) 1/25 1/25 1/25 1/25 .75/19 .75/19 S (in/mm) 2/51 2/51 2/51 1.5/38 2/51 2/51 Electrode Curr. (A) .91 n/m n/m n/m n/m n/m Total Curr. Draw (A) 6.36 6.25 5.59 5.93 3.57 3.71 Hydrodynamic r (nm) 12 16 16 12.5 13.9 14.2 TEM Avg. Dia. (nm) 10.42 12.06 11.11 12.06 11.74 13.02 “c-c” (mm) 76 76 76 76 n/a 76 Set electrode # 1a 1a 1a 1a n/a 1a 1 “x” (in/mm) 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 n/a 0.25/6.4 electrode # 5a 5a 5a 5a n/a 5a “c-c” (mm) 102 102 102 102 102 102 Set electrode # 5b 5b 5b 5b 5b 5b 2 “x” (in/mm) n/a n/a n/a n/a n/a n/a electrode # .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ .sup. 5b′ “c-c” (mm) 76 76 76 76 76 76 Set electrode # 5c 5c 5c 5c 5c 5c 3 electrode # .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ .sup. 5c′ “c-c” (mm) 76 76 76 76 76 76 Set electrode # 5d 5d 5d 5d 5d 5d 4 electrode # .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ .sup. 5d′ “c-c” (mm) 127 127 127 127 127 127 Set electrode # 5e 5e 5e 5e 5e 5e 5 electrode # .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ .sup. 5e′ “c-c” (mm) 127 127 127 127 127 127 Set electrode # 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 5f.sup. 6 electrode # 5f′ 5f′ 5f′ 5f′ 5f′ 5f′ “c-c” (mm) 152 152 152 152 152 152 Set electrode # 5g 5g 5g 5g 5g 5g 7 electrode # .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ .sup. 5g′ “c-c” (mm) 178 178 178 178 178 178 Set electrode # 5h 5h 5h 5h 5h 5h 8 electrode # .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ .sup. 5h′ “c-c” (mm) 76 76 76 76 76 76
[0684] All trough members 30a′ and 30b′ in the aforementioned
[0685] Table 7 shows that the processing enhancer NaHCO.sub.3 was added to purified water (discussed elsewhere herein) in amounts of either about 0.26 mg/ml or 0.53 mg/ml. It should be understood that other amounts of this processing enhancer (and other processing enhancers) also function within the metes and bounds of the invention. The purified water/NaHCO.sub.3 mixture was used as the liquid 3 input into trough member 30a′. The depth “d” of the liquid 3′ in the trough member 30a′ (i.e., where the plasma(s) 4 is/are formed) was about 7/16″ to about ½″ (about 11 mm to about 13 mm) at various points along the trough member 30a′. The depth “d′” was partially controlled through use of the dam 80 (shown in
[0686] The rate of flow of the liquid 3′ into the trough member 30a′ as well as into trough member 30b′, varied (as shown in Table 7) and the rate of flow out of the trough member 30b′ at the point 32 also varied due to different flow rate inputs and evaporation. Other acceptable flow rates should be considered to be within the metes and bounds of the invention.
[0687] Such flow of liquid 3′ was obtained by utilizing a Masterflex® L/S pump drive 40 rated at 0.1 horsepower, 10-600 rpm. The model number of the Masterflex® pump 40 was 77300-40. The pump drive had a pump head also made by Masterflex® known as Easy-Load Model No. 7518-10. In general terms, the head for the pump 40 is known as a peristaltic head. The pump 40 and head were controlled by a Masterflex® LS Digital Modular Drive. The model number for the Digital Modular Drive is 77300-80. The precise settings on the Digital Modular Drive were, for example, 150 milliliters per minute for all samples except GB-144 which was, for example, 110 ml/minute. Tygon® tubing having a diameter of ¼″ (i.e., size 06419-25) was placed into the peristaltic head. The tubing was made by Saint Gobain for Masterflex®. One end of the tubing was delivered to a first end 31 of the trough member 30′a by a flow diffusion means located therein. The flow diffusion means tended to minimize disturbance and bubbles in water 3 introduced into the trough member 30a′ as well as any pulsing condition generated by the peristaltic pump 40. In this regard, a small reservoir served as the diffusion means and was provided at a point vertically above the end 31 of the trough member 30a′ such that when the reservoir overflowed, a relatively steady flow of liquid 3′ into the end 31 of the V-shaped trough member 30a′ occurred.
[0688] Table 7 shows that there was a single electrode set 1a/5a, utilized in this Example 18. The plasma(s) 4 was/were created with an electrode 1 similar in shape to that shown in
[0689] The output from the trough member 30a′ was the conditioned liquid 3′ and this conditioned liquid 3′ flowed directly into a second trough member 30b′. The second trough member 30b′, shown in
[0690] Each electrode set 5a/5b was connected to a Chroma 61604 programmed AC power source (not shown and as discussed elsewhere herein). The applied voltages are reported in Table 7. Specifically, Table 7 refers to each of the electrode sets by “Set #” (e.g., “Set 1” through “Set 8”). Each electrode of the 1/5 or 5/5 electrode sets was set to operate within a specific voltage range. The voltages listed in Table 7 are the voltages used for each electrode set. The distance “c-c” (with reference to
[0691] All materials for the electrodes 1/5 were obtained from Hi-Rel Alloys having an address of 23. Lewis Street, Fort Erie, Ontario L2A2P6, Canada.
[0692]
[0693]
[0694] Energy absorption spectra were obtained for the samples in Example 18 by using UV-VIS spectroscopy. This information was acquired using a dual beam scanning monochromator system capable of scanning the wavelength range of 190 nm to 1100 nm. The Jasco V-530 UV-Vis spectrometer was used to collect absorption spectroscopy. Instrumentation was setup to support measurement of low-concentration liquid samples using one of a number of fused-quartz sample holders or “cuvettes.” The various cuvettes allow data to be collected at 10 mm, 1 mm or 0.1 mm optic path of sample. Data was acquired over the wavelength range using between 250-900 nm detector with the following parameters; bandwidth of 2 nm, with data pitch of 0.5 nm, a silicon photodiode with a water baseline background. Both deuterium (D2) and halogen (WI) scan speed of 400 nm/mm sources were used as the primary energy sources. Optical paths of these spectrometers were setup to allow the energy beam to pass through the center of the sample cuvette. Sample preparation was limited to filling and capping the cuvettes and then physically placing the samples into the cuvette holder, within the fully enclosed sample compartment. Optical absorption of energy by the materials of interest was determined. Data output was measured and displayed as Absorbance Units (per Beer-Lambert's Law) versus wavelength.
[0695] Spectral patterns in a UV-Visible range were obtained for each of the solutions/colloids produced in Example 18.
[0696] Specifically,
[0697]
[0698] In general, UV-Vis spectroscopy is the measurement of the wavelength and intensity of absorption of near-ultraviolet and visible light by a sample. Ultraviolet and visible light are energetic enough to promote outer electrons to higher energy levels. UV-Vis spectroscopy can be applied to molecules and inorganic ions or complexes in solution.
[0699] The UV-Vis spectra have broad features that can be used for sample identification but are also useful for quantitative measurements. The concentration of an analyte in solution can be determined by measuring the absorbance at some wavelength and applying the Beer-Lambert Law.
Example 19
Manufacturing Gold-Based Nanoparticles/Nanoparticle Suspensions or Colloids Aurora-002, Aurora-004, Aurora-006, Aurora-007, Aurora-009, Aurora-011, Aurora-012, Aurora-013, Aurora-014, Aurora-016, Aurora-017, Aurora-019, Aurora-020, Aurora-021, Aurora-022, Aurora-023, Aurora-024, Aurora-025, Aurora-026, Aurora-027, Aurora-028, Aurora-029 and Aurora-030
[0700] In general, Example 19 utilizes a trough member 30 and electrode 1/5 combination different from any of the other Examples disclosed herein. Specifically, this Example utilizes a first set of four electrodes 1 and a single electrode 5a in a trough member 30a′ which create a plurality of plasmas 4, resulting in conditioned liquid 3′. The conditioned liquid 3′ flows into and through a longitudinal trough member 30b′, wherein parallelly located electrodes 5b/5b′ are positioned along substantially the entire longitudinal or flow length of the trough member 30b′. Specific reference is made to
TABLE-US-00022 TABLE 8 Aurora- Aurora- Aurora- Aurora- Aurora- Run ID: 002 004 006 007 009 Flow Rate: In (ml/min) 300 300 150 150 150 Volts: Set # 1 1000 1000 1000 1000 1000 Electrodes 5b 100 120 100 50 100 # of Electrodes 1 4 4 4 4 4 PE: NaHCO3 (mg/ml) 0.396 0.396 0.396 0.396 0.396 Wire Diameter (mm) 0.5 0.5 0.5 0.5 0.5 Electrode Config. FIG. 23a 23a 23a 23a 23a Produced Au PPM 12.3 15.9 39.6 4.1 17.8 Dimensions Plasma 4 FIGS. 23a 23a 23a 23a 23a Process FIGS. 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23c, 23d 23c, 23d 23c, 23d 23c, 23d 23c, 23d Wire Length (in) 54 54 54 54 54 “W.sub.L” L.sub.T (in/mm) 59/1500 59/1500 59/1500 59/1500 59/1500 wire apart 0.125/3.2 0.125/3.2 0.125/3.2 0.125/3.2 0.125/3.2 (in/mm) “b” Electrode Curr. (A) 10.03 14.2 15.3 5.2 11.9 Hydrodynamic r (nm) 23.2 19.4 23.2 26.2 19.6 TEM Avg. Dia. (nm) n/a n/a n/a n/a n/a Aurora- Aurora- Aurora- Aurora- Run ID: 011 012 013 014 Flow Rate: In (ml/min) 300 450 60 60 Volts: Set # 1 1000 1000 1000 1000 Electrodes 5b 90 110 50 40 # of Electrodes 1 4 4 4 4 PE: NaHCO3 (mg/ml) 0.396 0.396 0.396 0.396 Wire Diameter (mm) 0.5 0.5 0.5 0.5 Electrode Config. FIG. 23a 23a 23a 23a Produced Au PPM 17.4 12.7 46.5 65.7 Dimensions Plasma 4 FIGS. 23a 23a 23a 23a Process FIGS. 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23c, 23d 23c, 23d 23c, 23d 23c, 23d Wire Length (in) 54 54 54 54 “W.sub.L” L.sub.T (in/mm) 59/1500 59/1500 59/1500 59/1500 wire apart 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 (in/mm) “b” Electrode Curr. (A) 15.9 19.5 10 7.87 Hydrodynamic r (nm) 16.3 13.1 26.2 22.0 TEM Avg. Dia. (nm) n/a n/a n/a n/a Aurora- Aurora- Aurora- Aurora- Aurora- Run ID: 016 017 019 020 021 Flow Rate: In (ml/min) 60 30 30 30 30 Volts: Set # 1 1000 1000 1000 1000 1000 Electrodes 5b 30 30 30 50 50 # of Electrodes 1 4 4 1 1 4 PE: NaHCO3 (mg/ml) 0.396 0.396 0.396 0.396 0.396 Wire Diameter (mm) 0.5 0.5 0.5 0.5 0.5 Electrode Config. FIG. 23a 23a 23a 23a 23a Produced Au PPM 35.5 24.8 22.5 128.2 67.1 Dimensions Plasma 4 FIGS. 23a 23a 23a 23a 23a Process FIGS. 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23c, 23d 23c, 23d 23c, 23d 23c, 23d 23c, 23d Wire Length (in) 54 54 54 54 54 “W.sub.L” L.sub.T (in/mm) 59/1500 59/1500 59/1500 59/1500 59/1500 wire apart 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 (in/mm) “b” Electrode Curr. (A) 5.18 4.95 4.65 10.7 10 Hydrodynamic r (nm) 26.6 27.4 26.0 31.0 27.1 TEM Avg. Dia. (nm) n/a n/a n/a 16-40 n/a Aurora- Aurora- Aurora- Aurora- Run ID: 022 023 024 025 Flow Rate: In (ml/min) 60 60 60 60 Volts: Set # 1 1000 1000 1000 1000 Electrodes 5b 50 80 30 30 # of Electrodes 1 4 4 4 4 PE: NaHCO3 (mg/ml) 0.396 0.396 3.963 3.963 Wire Diameter (mm) 0.5 0.5 0.5 0.5 Electrode Config. FIG. 23a 23a 23a 23a Produced Au PPM 64.2 73.8 0.8 0.5 Dimensions Plasma 4 FIGS. 23a 23a 23a 23a Process FIGS. 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23c, 23d 23c, 23d 23c, 23d 23c, 23d Wire Length (in) 54 50 50 50 “W.sub.L” L.sub.T (in/mm) 59/1500 59/1500 59/1500 59/1500 wire apart 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 (in/mm) “b” Electrode Curr. (A) 9.8 18 17 14.96 Hydrodynamic r (nm) 28.3 27.0 n/a n/a TEM Avg. Dia. (nm) n/a n/a n/a n/a Aurora- Aurora- Aurora- Aurora- Aurora- Run ID: 026 027 028 029 030 Flow Rate: In (ml/min) 60 60 60 60 60 Volts: Set # 1 1000 1000 1000 1000 1000 Electrodes 5b 30 30 100 130 150 # of Electrodes 1 4 4 4 4 4 PE: NaHCO3 (mg/ml) 3.963 3.963 0.106 0.106 0.106 Wire Diameter (mm) 0.5 0.5 0.5 0.5 0.5 Electrode Config. FIG. 23a 23a 23a 23a 23a Produced Au PPM 3.7 2.0 8.1 21.6 41.8 Dimensions Plasma 4 FIGS. 23a 23a 23a 23a 23a Process FIGS. 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23a, 23b, 23c, 23d 23c, 23d 23c, 23d 23c, 23d 23c, 23d Wire Length (in) 50 50 50 50 50 “W.sub.L” L.sub.T (in/mm) 59/1500 59/1500 59/1500 59/1500 59/1500 wire apart 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 0.063/1.6 (in/mm) “b” Electrode Curr. (A) 13.4 16.32 6.48 10 12 Hydrodynamic r (nm) 33.7 and n/a 26.1 21.9 25.2 77.5 TEM Avg. Dia. (nm) n/a n/a n/a n/a n/a
[0701] With regard to
[0702] Only one set of electrodes 5b/5b′ was utilized in this particular embodiment. These electrodes 5b/5b′ were connected to an AC power source 50, as described in the other Examples herein. The gold wire electrodes 5b/5b′ used in this particular Example were the same gold wires, with dimensions as reported in Table 8, that were used in the other Examples reported herein. However, a relatively long length (i.e., relative to the other Examples herein) of gold wire electrodes was located along the longitudinal length L.sub.T of the trough member 30b′. The wire length for the electrodes 5b/5b′ is reported in Table 8. Two different wire lengths either 50 inches (127 cm) or 54 inches (137 cm) were utilized. Further, different transverse distances between the wires 5b/5b′ are also reported. Two separate transverse distances are reported herein, namely, 0.063 inches (1.6 mm) and 0.125 inches (3.2 mm). Different electrode 5b/5b′ lengths are utilizable as well as a plurality of different transverse distances between the electrodes 5b/5b′.
[0703] The wire electrodes 5b/5b′ were spatially located within the liquid 3″ in the trough member 30b′ by the devices Gb, Gb′, T8, T8′, Tb and Tb′ near the input end 31 (refer to
[0704] Table 8 shows a variety of relevant processing conditions, as well as certain results including, for example, “Hydrodynamic r” (i.e., hydrodynamic radii (reported in nanometers)) and the process current that was applied across the electrodes 5b/5b′. Additionally, resultant ppm levels are also reported for a variety of process conditions with a low of about 0.5 ppm and a high of about 128 ppm.
[0705]
[0706]
[0707]
[0708] Accordingly, it is clear from this continuous processing method that a variety of process parameters can influence the resultant product produced.
Example 20
Manufacturing Gold-Based Nanoparticles/Nanoparticle Suspensions or Colloids GA-002, GA-003, GA-004, GA-005, GA-009, GA-011 and GA-013 by a Batch Process
[0709] This Example utilizes a batch process according to the present invention.
TABLE-US-00023 TABLE 9 Run ID: GA-002 GA-003 GA-004 GA-005 GA-009 GA-011 GA-013 Dwell Plasma 4 25 25 25 25 25 25 25 Times Electrodes 42 42 42 42 42 42 42 (min) 5a/5b Volume Plasma 4 3790 3790 3790 3790 3790 3790 3790 H.sub.2O & PE Electrodes 900 900 900 900 900 900 900 (mL) 5a/5b Volts: Plasma 4 750 750 750 750 750 750 750 Electrodes 300 300 300 300 298 205.6 148 5a/5b PE* Type: Na.sub.2CO.sub.3 K.sub.2CO.sub.3 KHCO.sub.3 NaHCO.sub.3 NaHCO.sub.3 NaHCO.sub.3 NaHCO.sub.3 mg/ml: 0.22 0.29 0.44 0.47 0.52 0.51 0.51 Wire Diameter (mm) 1.0 1.0 1.0 1.0 1.0 1.0 1.0 Wire Configuration FIG. 17b 17b 17b 17b 17b 17b 17b PPM: 7.8 10.0 10.0 11.3 9.7 10.0 7.7 Final Liquid Temp ° C. 96 93.5 90.5 89 90.5 74.5 57 Dimensions & Plasma 4 24a 24a 24a 24a 24a 24a 24a Configuration FIG. Electrodes 24c 24c 24c 24c 24c 24c 24c 5a/5b FIG. Contact “W.sub.L” 0.75/19 0.75/19 0.75/19 0.75/19 0.75/19 0.75/19 0.75/19 (in/mm) Separation 1.5/38 1.5/38 1.5/38 1.5/38 1.5/38 0.25/6 0.063/1.6 (in/mm) Electrode Current (A) 0.69 0.65 0.64 0.66 0.76 0.78 0.60 Hydrodynamic r (nm) 11.1 12.0 13.9 11.9 17.6 17.1 10.3 TEM Avg. Diameter (nm) 12.24 12.74 14.09 14.38 11.99 11.99 11.76 “c-c” (in/mm) n/m n/m n/m n/m n/m n/m n/m Plasma 4 electrode # 1a 1a 1a 1a 1a 1a 1a “x” (in/mm) 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 0.25/6.4 electrode # 5a 5a 5a 5a 5a 5a 5a “c-c” (in/mm) n/m n/m n/m n/m n/m n/m n/m Electrodes electrode # 5a 5a 5a 5a 5a 5a 5a electrode # 5b 5b 5b 5b 5b 5b 5b
[0710] With regard to the reported processing enhancers (PE) utilized, different mg/ml amounts were utilized in an effort to have similar conductivity for each solution (e.g., also similar molar quantities of cations present in the liquid 3/3′). The electrode wire diameter used in each Example was the same, about 1.0 mm, and was obtained from ESPI, having an address of 1050 Benson Way, Ashland, Oreg. 97520, as reported elsewhere herein.
[0711] The amount of electrode contacting the liquid 3′ in the apparatus shown in
[0712] Table 9 also shows the effects of transverse electrode separation (i.e., the distance “b” between substantially parallel electrodes 5a/5b shown in
[0713] A voltage source 60 (discussed elsewhere herein) was used to create the plasma 4 shown in
[0714] Table 9 also reports the measured hydrodynamic radius (i.e., a single number for “Hydrodynamic Radii” taken from the average of the three highest amplitude peaks shown in each of
[0715]
[0716]
[0717]
Comparative Example 21
Manufacturing Gold-Based Nanoparticles/Nanoparticle Suspensions According to the Bredig/Svedberg Processes
[0718] This Example utilizes an underwater AC plasma created between two gold electrodes in an attempt to make a gold nanoparticle suspension similar to those made by Bredig and Svedberg (discussed in the Background).
[0719] Specifically,
[0720]
Comparative Example 22a
Colloidal-Based Nanoparticle Suspensions Commercially Available
[0721] For comparison purposes, eight commercially available colloidal gold solutions were obtained. The commercial names and sources are listed in Table 10 below:
TABLE-US-00024 TABLE 10 Solution Name Manufacturer Description Utopia Gold Utopia Silver Supplements Colloidal Gold SNG911219 Source Naturals, Inc. Ultra Colloidal Gold Nanopartz Nanopartz Accurate Spherical Gold Nanoparticles Nanocomposix NanoComposix Tannic Acid 15 nm NanoXact Gold Nanocomposix NanoComposix Tannic NanoXact 10 nm Gold Harmonic Gold Harmonic Innerprizes ElectraClear InSpiral Technologies Colloidal Gold MesoGold Purest Colloids, Inc.
[0722]
[0723]
Particle-Size and Particle-Shape Analysis
[0724] Transmission electron microscope (TEM) images were analyzed by visual observation with the aid of software referenced in Examples 5-7. Individual particles/crystals were assigned to one of five groups according to the two-dimensional projection shown in the photomicrographs. The five categories are: triangle, pentagon, hexagon, diamond and other. These categories correspond to three-dimensional morphologies elucidated in the literature and prior TEM studies which utilized a tilting sample holder. The 2D/3D correspondence of the particle/crystal shape categories is listed in Table 11.
TABLE-US-00025 TABLE 11 Two-Dimensional Possible Three-Dimensional Nanoparticle Projection Morphologies Triangle Tetrahedron Pentagon Pentagonal Bipyramid (i.e., Decahedron) Hexagon Hexagonal Bipyramid, Icosahedrons, Octahedron Diamond Octahedron, Various Elongated Bipyramids, Fused Tetrahedrons, Side View of Bipyramids Other Icosahedrons, Spheroids, Ellipsoids, Rods, Aggre- gated Particles, Platelets, Particles of Uncertain Form
[0725] Certain nanocrystal forms can take on multiple two-dimensional projections. For example, an icosahedron, a possible shape for gold nanocrystals, can appear as a hexagon, an irregular heptagon or a spheroid in a TEM micrograph. While care was taken to discern the hexagonal, octagonal and other shapes when viewed in the two-dimension projection, conclusive information regarding the true form of such nanocrystals cannot always be discerned in the two-dimensional projection. Therefore, only the tetrahedron and pentagonal bipyramid (i.e., decahedron) categories can be absolutely discerned. Hexagonal, Diamond and Other categories are grouped together.
[0726] A pentagonal bipyramid nanocrystal viewed on its side could be projected as a diamond. This is an unlikely occurrence given the planar nature of the sample substrate and taking into consideration the very low number of diamonds counted throughout the analysis. Those decahedrons counted via the pentagon two-dimensional projection are distinct from this former group, per se, and their count was taken as one a figure of merit or method of distinguishing the inventive crystals from those of the art. Likewise, triangles or tetrahedrons are also readily distinguishable and can also be used for comparison purposes.
[0727] Aggregation and agglomeration of particles or nanocrystals can occur in a colloid or as an artifact of the drying process required for TEM sample preparation/analysis. Dense agglomerations and larger aggregations (greater than approximately 50 particles/nanocrystals) were not analyzed due to possible counting errors. The crystal/particle number and particle/crystal shapes of smaller aggregates and visually resolvable agglomerations were analyzed. Additionally, only well resolved images were used for this investigation.
[0728] In order to be very conservative, during the analysis of TEM micrographs of all suspensions or colloids produced according of the invention, any questionable crystals were assigned to the group labeled “Other”. Questionable crystals were those that possibly belong to a well-defined crystal categories, but some uncertainty exists (e.g., a small pentagon with one corner obscured by an adjacent particle). In contrast, when performing the analysis of the particles in the commercially available colloids, any particle of questionable shape was given “the benefit of the doubt” and was assigned to the “category “Hexagonal” despite the uncertainty of its actual crystal structure. Thus the crystal/particle shape comparisons are not biased and are very conservative regarding possible differences between commercially available colloids and nanocrystalline colloids made according to the invention.
[0729] It is clear from Table 12 that the presence of nanocrystals corresponding in shape to pentagonal bipyramids and/or tetrahedrons is/are quite different from the commercially available colloids and ARCG-05. Moreover, these nanocrystals have substantially “clean” surfaces, as discussed, shown and defined elsewhere herein.
TABLE-US-00026 TABLE 12 TEM Average Example Pentagonal Other Diameter Product Number Bipyramid Tertrahedron Octahedron Hexagonal Shapes PPM (nm) pH GD-007 5 21% 10% 2% 40% 27% 14 14.3 8.9 GB-056 17 34% 13% 6% 30% 17% 12 12.1 9.1 GB-077 16 22% 8% 3% 40% 27% 8 8.7 9.0 GB-134 16 31% 18% 5% 27% 19% 9 17.5 9.2 GB-151 18 32% 8% 5% 36% 19% 8 10.9 9.4 GB-154 13 14% 7% 4% 23% 51% 5 14.1 9.7 GB-156 13 18% 16% 5% 30% 30% 5 19.4 9.2 GB-162 14 15% 32% 1% 16% 37% 8 8.9 9.0 GB-163 15 9% 21% 2% 28% 40% 8 20.6 9.1 GB-164 15 12% 12% 7% 32% 37% 8 20.4 9.3 GB-165 14 22% 19% 5% 24% 30% 7 14.7 9.0 GB-166 14 15% 10% 2% 24% 49% 6 13.0 9.0 GB-175 18 25% 22% 1% 23% 29% 11 11.8 9.3 GB-176 18 23% 20% 1% 35% 21% 10 10.4 9.3 GB-177 18 29% 19% 1% 28% 23% 10 10.9 9.3 GB-188 18 25% 23% 6% 23% 24% 8 10.6 9.1 GB-189 18 26% 21% 0% 23% 30% 8 10.4 9.2 GB-194 18 22% 19% 3% 33% 23% 9 12.1 9.2 GB-195 18 17% 16% 3% 45% 19% 8 11.1 9.2 GB-196 18 21% 16% 1% 31% 30% 9 12.1 9.1 GB-198 18 14% 10% 0% 51% 25% 10 11.7 9.2 GB-199 18 33% 9% 1% 40% 17% 12 13.0 9.1 GA-002 20 30% 23% 5% 24% 18% 11 12.2 10.5 GA-003 20 27% 17% 6% 32% 18% 10 12.7 10.3 GA-004 20 15% 9% 3% 38% 35% 10 14.1 9.0 GA-005 20 14% 13% 4% 31% 37% 11 14.4 9.1 GA-009 20 11% 11% 2% 36% 39% 10 12.0 9.2 GA-011 20 8% 6% 6% 37% 44% 10 12.0 8.9 GA-013 20 8% 13% 5% 28% 48% 8 11.8 8.7 GT-033 1-4 4% 1% 1% 26% 68% 2 11.8 6.7 1AC-261-1 12 12% 12% 2% 37% 37% 14 12.2 AURORA 020 19 15% 14% 1% 31% 39% 128 20.6 9.0 ARCG-05 21 3% 0% 2% 6% 89% 5 13.7 6.3 Utopia Gold 22 5% 2% 1% 5% 89% 9 4.7 5.1 SNG911219 22 2% 0% 0% 11% 87% 13 18.4 6.9 Nanopartz 22 2% 0% 0% 21% 77% 39 21.9 7.6 Nanocomposix 22 3% 4% 2% 10% 81% 49 17.8 5.2 15 nm Nanocomposix 22 2% 1% 1% 22% 73% 51 13.7 5.1 10 nm Harmonic Gold 22 8% 2% 2% 35% 55% 5 8.9 8.8 ElectraClear 22 6% 2% 2% 20% 71% 3 5.7 6.3 MesoGold 22 5% 1% 2% 15% 78% 20 8.5 5.7
Example 22b
The Zeta Potential Example
[0730] The nature and/or amount of the surface change (i.e., positive or negative) on formed nanoparticles can also have a large influence on the behavior and/or effects of the nanoparticle/suspension or colloid. For example, a protein corona can be influenced by surface change on a nanoparticle. Such surface changes are commonly referred to as “zeta potential”. In general, it is well known that the larger the zeta potential (either positive or negative), the greater the stability of the nanoparticles in the solution (i.e., the suspension is more stable). However, by controlling the nature and/or amount of the surface charges of formed nanoparticles the performance of such nanoparticle solutions in a variety of systems can be controlled. It should be clear to an artisan of ordinary skill that slight adjustments of chemical composition, reactive atmospheres, power intensities, temperatures, etc., can cause a variety of different chemical compounds (both semi-permanent and transient) nanoparticles (and nanoparticle components) to be formed, as well as different nanoparticle/solutions (e.g., including modifying the structures of the liquid 3 (such as water) per se). Accordingly, this Example measures the zeta potential of several suspensions made according to the invention, as well as several commonly available colloidal gold suspensions.
[0731] “Zeta potential” is known as a measure of the electo-kinetic potential in colloidal systems. Zeta potential is also referred to as surface charge on particles. Zeta potential is also known as the potential difference that exists between the stationary layer of fluid and the fluid within which the particle is dispersed. A zeta potential is often measured in millivolts (i.e., mV). The zeta potential value of approximately 25 mV is an arbitrary value that has been chosen to determine whether or not stability exists between a dispersed particle in a dispersion medium. Thus, when reference is made herein to “zeta potential”, it should be understood that the zeta potential referred to is a description or quantification of the magnitude of the electrical charge present at the double layer.
[0732] The zeta potential is calculated from the electrophoretic mobility by the Henry equation:
where z is the zeta potential, U.sub.E is the electrophoretic mobility, ε is a dielectric constant, η is a viscosity, f(ka) is Henry's function. For Smoluchowski approximation f(ka)=1.5.
[0733] Electrophoretic mobility is obtained by measuring the velocity of the particles in an applied electric field using Laser Doppler Velocimetry (“LDV”). In LDV the incident laser beam is focused on a particle suspension inside a folded capillary cell and the light scattered from the particles is combined with the reference beam. This produces a fluctuating intensity signal where the rate of fluctuation is proportional to the speed of the particles (i.e. electrophoretic mobility).
[0734] In this Example, a Zeta-Sizer “Nano-ZS” produced by Malvern Instruments was utilized to determine zeta potential. For each measurement a 1 ml sample was filled into clear disposable zeta cell DTS1060C. Dispersion Technology Software, version 5.10 was used to run the Zeta-Sizer and to calculate the zeta potential. The following settings were used: dispersant—water, temperature—25° C., viscosity—0.8872 cP, refraction index—1.330, dielectric constant—78.5, approximation model—Smoluchowski. One run of hundred repetitions was performed for each sample.
[0735]
[0736]
Example 23a
[0737] This Example 13a utilized a set of processing conditions similar to those set forth in Examples 5-7. This Example utilized an apparatus similar to those shown in
TABLE-US-00027 TABLE 13 0.528 mg/ml of NaHCO.sub.3 (Au) Run ID: GD-006 Flow Rate: 240 ml/min Voltage: 255 V NaHCO.sub.3: 0.528 mg/ml Wire Dia.: .5 mm Configuration: Straight/Straight PPM: 8.7 Distance Distance Elec- “c-c” “x” Volt- cross Set# trode# in/mm in/mm age section 4.5/114.3* 1 1a 0.25 750 V 5a N/A 750 23/584.2** 2.5/63.5* 2 5b N/A 255 .sup. 5b′ N/A 8.5/215.9 3 5c N/A 255 Rectangle .sup. 5c′ N/A 5.25″ 8.5/215.9 Deep 4 5d N/A 255 .sup. 5d′ N/A .sup. 8/203.2 5 5e N/A 255 .sup. 5e′ N/A 2/50.8** Output Water Temperature 95 C. *Distance from water inlet to center of first electrode set **Distance from center of last electrode set to water oulet
[0738]
Example 23b
[0739] This Example 23b utilized the suspension of Example 23a to manufacture a gel or cream product. Specifically, about 1,300 grams of the suspension made according to Example 13a was heated to about 60° C. over a period of about 30 minutes. The suspension was heated in a 1-liter Pyrex® beaker over a metal hotplate. About 9.5 grams of Carbopol® (ETD 2020, a carbomer manufactured by Noveon, Inc., Cleveland, Ohio) was added slowly to the heated suspension, while constantly stirring using a squirrel rotary plastic paint mixer. This mixing occurred for about 20 minutes until large clumps of the Carbopol were dissolved.
[0740] About 15 grams of high purity liquid lanolin (Now Personal Care, Bloomingdale, Ill.) was added to the suspension and mixed with the aforementioned stirrer.
[0741] About 16 grams of high purity jojoba oil were then added and mixed to the suspension.
[0742] About 16 grams of high purity cocoa butter chunks (Soap Making and Beauty Supplies, North Vancouver, B.C.) were heated in a separate 500 mL Pyrex® beaker and placed on a hotplate until the chunks became liquid and the liquid cocoa butter then was added and mixed to the aforementioned suspension.
[0743] About 16 grams of potassium hydroxide (18% solution) was then added and mixed together with the aforementioned ingredients to cause the suspension to gel. The entire suspension was thereafter continuously mixed with the plastic squirrel rotating mixer to result in a cream or gel being formed. During this final mixing of about 15 minutes, additional scent of “tropical island” (2 mL) was added. The result was a pinkish, creamy gel.
Example 23c
[0744] This Example 23c utilized the suspension made according to Example 7. Specifically, this Example utilized the product of Example 7 (i.e., GD-015) to manufacture a gel or cream product. Specifically, about 650 grams of the solution made according to Example 7 was heated to about 60° C. over a period of about 30 minutes. The suspension was heated in a Iliter Pyrex® beaker over a metal hotplate. About 9.6 grams of Carbopol® (ETD 2020, a carbomer manufactured by Noveon, Inc., Cleveland, Ohio) was added slowly to the heated suspension, while constantly stirring using a squirrel rotary plastic paint mixer. This mixing occurred for about 20 minutes until large clumps of the carbopol were dissolved.
[0745] About 7 grams of high purity liquid lanolin (Now Personal Care, Bloomingdale, Ill.) was added to the solution and mixed with the aforementioned stirrer.
[0746] About 8 grams of high purity jojoba oil were then added and mixed to the suspension.
[0747] About 8 grams of high purity cocoa butter chunks (Soap Making and Beauty Supplies, North Vancouver, B.C.) were heated in a separate 500 mL Pyrex® beaker and placed on a hotplate until the chunks became liquid and the liquid cocoa butter then was added and mixed to the aforementioned suspension.
[0748] About 45 grams of the liquid contained in Advil® liquid gel caps (e.g., liquid ibuprofen and potassium) was added to, and thoroughly mixed with, the suspension.
[0749] About 8 grams of potassium hydroxide (18% solution) was then added and mixed in to cause the suspension to gel. The entire solution was thereafter continuously mixed with the plastic squirrel rotating mixer to result in a cream or gel being formed. During this final mixing of about 15 minutes, additional scent of “tropical island” (2 mL) was added. The result was a pinkish, creamy gel.
Example 23d
[0750] This Example 23d utilized suspension equivalent to GB-139 to manufacture a gel or cream product. Specifically, about 650 grams of the suspension was heated to about 60° C. over a period of about 30 minutes. The suspension was heated in a 1-liter Pyrex® beaker over a metal hotplate. About 6 grams of Carbopol® (ULTREZ10, a carbomer manufactured by Noveon, Inc., Cleveland, Ohio) was added slowly to the heated suspension, while constantly stirring using a squirrel rotary plastic paint mixer. This mixing occurred for about 20 minutes until large clumps of the Carbopol were dissolved.
[0751] About 7 grams of high purity liquid lanolin (Now Personal Care, Bloomingdale, Ill.) was added to the suspension and mixed with the aforementioned stirrer.
[0752] About 8 grams of high purity jojoba oil were then added and mixed to the suspension.
[0753] About 8 grams of high purity cocoa butter chunks (Soap Making and Beauty Supplies, North Vancouver, B.C.) were heated in a separate 500 mL Pyrex® beaker and placed on a hotplate until the chunks became liquid and the liquid cocoa butter then was added and mixed to the aforementioned suspension.
[0754] About 8 grams of potassium hydroxide (18% solution) was then added and mixed together with the aforementioned ingredients to cause the suspension to gel. The entire suspension was thereafter continuously mixed with the plastic squirrel rotating mixer to result in a cream or gel being formed. The result was a pinkish, creamy gel.
Example 23e
[0755] This Example 23e utilized a suspension substantially equivalent to 1AC-261 to manufacture a gel or cream product. Specifically, about 450 grams of the suspension was heated to about 60° C. over a period of about 30 minutes. The suspension was heated in a 1-liter Pyrex® beaker over a metal hotplate. About 4.5 grams of Carbopol® (ULTREZ10, a carbomer manufactured by Noveon, Inc., Cleveland, Ohio) was added slowly to the heated suspension, while constantly stirring using a squirrel rotary plastic paint mixer. This mixing occurred for about 20 minutes until large clumps of the Carbopol were dissolved.
[0756] About 6.5 grams of potassium hydroxide (18% solution) was then added and mixed together with the aforementioned ingredients to cause the suspension to gel. The entire suspension was thereafter continuously mixed with the plastic squirrel rotating mixer to result in a cream or gel being formed. The result was a pinkish, creamy gel.
Example 24
In Vitro Study of the Effects of Gold Nanocrystalline Formulation GB-079 on Monocyte Cytokine Production
Summary
[0757] This in vitro Example was designed to determine the effects of gold nanocrystalline suspension GB-079 on four different cytokines/chemokines. Specifically in this Example, human peripheral blood mononuclear cells (“hPBMC”) were cultured in the presence or absence of each of four different concentration or ppm levels of gold nanocrystalline suspension GB-079 (i.e., a suspension or colloid made in accordance with the disclosure of one example herein) in the presence or absence of (as disclosed herein) bacterial lipopolysaccharide (“LPS”).
[0758] It is known that lipopolysaccharide binds to TLR4, a receptor expressed on a number of different immune system cells, and such binding typically triggers activation and/or expression of a series of cytokines, typically in an NFkB-dependent (i.e., Nuclear Factor kB-dependent) manner. After about 24 hours of culture conditions at about 37° C. in about 5% CO.sub.2 and a humidified atmosphere of about 95% relative humidity, supernatants were removed and assayed for the presence of a series of different cytokines/chemokines, including: MIF, TNFα, IL-6 and IL-10. The majority of, but not the only source of, these cytokines in the hPBMC population would be expected to be monocytes. Cultures in the absence of LPS indicate whether treatments induce the production of these cytokines/chemokines, while those cultures in the presence of LPS will indicate whether treatments are able to modulate the production of cytokines in response to an inflammatory stimulus. Cytokine assays were performed by the Luminex® Extracellular Assay Protocol. The Luminex system uses antibody coated microspheres that bind specifically to the cytokine being assayed. When excited by laser light the microspheres that have bound the antigen are measured and this is a direct assessment of the amount of the cytokine being produced and data were provided as raw data and absolute quantities of each cytokine/chemokine measured.
Preparation of hPBMC
Materials Used for Cell Preparation:
[0759]
TABLE-US-00028 Supplier Cat. No. PBMC Isolation Histopaque 1077 Sigma H8889 RPMI 1640 × 10 Sigma R1145 Endotoxin-free water (EFW) Gibco 15230-170 50 ml falcon tubes Corning 430829 Citrate ACD Sigma C3821-50 ml AB serum National Blood Service Plastic 24 well plates Costar/Corning 3524 LPS Sigma Media supplements Penicillin/streptomycin Sigma P0871 HEPES Sigma H0887 Glutamine Gibco 25030-024 Sodium Bicarbonate (7.5%) Gibco 25080
Equipment
[0760] NucleoCounter (i.e., cell number and viability counter made by Chemometec)
Benchtop centrifuge
Tissue culture hood
Collection of Human Blood
[0761] Blood from a healthy volunteer was drawn into a syringe and placed into a 50 ml falcon tube.
3.3 ml citrate anticoagulant (ACD, Sigma) was added to the 50 ml falcon tubes in a sterile manner.
Tubes were inverted to mix.
Cell Preparation Method
[0762] 1. 10×RPMI+supplements (25 ml 10×RPMI+2.5 ml Penstrep+2.5 ml L-glutamine+5 ml HEPES+6.7 ml sodium bicarbonate solution (7.5%)) were mixed together in a falcon tube, herein referenced to as the “culture media”. [0763] 2. Blood was resuspended in an equal volume of 1×RPMI 1640 (diluted from 10×RPMI in EFW—200 ml prepared [20 ml in 180 ml]) and mixed by inversion in a falcon tube. [0764] 3. The histopaque was prewarmed to room temperature (RT) and 20 ml was added to a 50 ml falcon tube. [0765] 4. The histopaque was gently overlayed with 30 ml blood/medium then mixed in. [0766] 5. The histopaque blood mix sample was spun at 1600 rpm in a benchtop centrifuge for about 25 min at RT (no brake). [0767] 6. PBMC were separated into the interface layer between the medium and the histopaque, cells were removed by aspriation into a 50 ml falcon tube and 10 ml of the culture media was added thereto. [0768] 7. The cell sample was spun at 1800 rpm for about 10 minutes at RT. [0769] 8. The cell sample was washed twice with 30 ml RPMI and resuspended in culture medium (RPMI, supplemented as described above=RPMI/no serum). [0770] 9. During the spin, RPMI supplemented with 5% AB serum was prepared. [0771] 10. The cell sample was resuspended in 2 ml RPMI+supplements+serum. [0772] 11. Cell counts were completed and viability assessment was performed using the Nucleocounter (i.e., a cell viability counter). [0773] 12. Cells were resuspended in 1×RPMI to give a final concentration of 2.5×10.sup.6 cells/ml. [0774] 13. 500 μl of cells were transferred into a 24-well plate. [0775] 14. 10×RPMI+supplements (500 μl PenStrep, 500 μl L-Glutamine, lml HEPES, 2.5 ml AB serum) was prepared by mixing together in a falcon tube, thereby forming the “test media”. [0776] 15. The inventive GB-079 gold nanocrystal suspension was added to the wells in the 24 well plate (900 μl total volume) [0777] 16. 100 μl 10×RPMI+supplements were added to each well of a costar 24 well plate. [0778] 17. The 24 well plates were placed into a humidified incubator set at 37° C./5% CO.sub.2 for 1 hour. [0779] 18. LPS was prepared at 4× final concentration in 1×RPMI [0780] 19. 500 μl of LPS was added per well, or 500 μl media to wells not receiving LPS, bringing the total well volume of material to each well to 2 ml. [0781] 20. Plates were placed into a humidified incubator set at 37° C./5% CO.sub.2 for about 24 hours. [0782] 21. 1800 μl (3×600 μl aliquots) of supernatant were removed for ELISA analysis and Luminex analysis. [0783] 22. Supernatants were stored at −80° C. until assayed in the Luminex® system.
Luminex® Assay System
[0784] The supernatants were assayed in accordance with the Luminex® Extracellular Assay Protocol, accessed on Jan. 11, 2010.
TABLE-US-00029 TABLE 14 Sample Compound EFW 10x RPMI Cells LPS 1x RPMI Cells + Vehicle 900 μl 100 μl 500 μl 500 μl Cells + Vehicle + LPS 900 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:5 400 μl 500 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:10 200 μl 700 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:20 100 μl 800 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:40 50 μl 850 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:100 20 μl 880 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:5 + LPS 400 μl 500 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:10 + LPS 200 μl 700 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:20 + LPS 100 μl 800 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:40 + LPS 50 μl 850 μl 100 μl 500 μl 500 μl Cells + [Test].sub.1:100 + LPS 20 μl 880 μl 100 μl 500 μl 500 μl
[0785] Cells were stimulated with LPS (a high dose of lmg/ml and a low dose of 10 ng/ml), the supernatants were then collected after 24 hours and analyzed for the amounts present of the 4 cytokines discussed herein. Control wells contained cells and the inventive test compound GB-079 but no LPS. Results obtained for each of the other cytokines/chemokines are shown in
[0786]
[0787]
[0788]
[0789] Further,
Example 25
Collagen Induced Arthritis (CIA) Study in Mice
Summary
[0790] This Example demonstrates the efficacy of two of the inventive gold nanocrystalline compositions (i.e., GT033 and GD-007) in a mouse CIA model. Specifically, male DBA/l mice (12 weeks old) were given 100 μg Chicken Type II collagen emulsified into complete Freund's adjuvant (“CII/CFA”) on day 0 of the study by injection at the base of the tail. Clinical joint swelling was scored three times weekly from day 14 until termination at day 42. Those results are summarized in
Methodology
Animals
[0791] Species: Mice [0792] Strain: DBA/1 [0793] Source: Harlan [0794] Gender and number: Male, 30 [0795] Age: About 12 weeks old at the start of the study. [0796] Identification: Each mouse was given a unique identity number. [0797] Animal husbandry: On receipt, all animals were examined for external signs of ill-health and all unhealthy animals were excluded from further evaluation. Animals were housed in groups of five under specific pathogen free (spf) conditions, in a thermostatically monitored room (22±4° C.) in an animal unit. Animals were equilibrated under standard animal house conditions for at least 72 hours prior to use. The health status of the animals was monitored throughout this period and the suitability of each animal for experimental use was assessed prior to study start. [0798] Housing Animals were housed in groups of 10 per cage in a controlled room, to ensure correct temperature, humidity and 12-hour light/dark cycle for the duration of the study. [0799] Diet: Irradiated pellet diet and water was available ad libitum throughout the holding, acclimatization and post-dose periods.
Compound and Reagents
Chicken Collagen Type II (Sigma, C9301).
Incomplete Freund's Adjuvant (“IFA”) (Sigma, FF5506)
[0800] Mycobacterium tuberculosis H37Ra (BD Biosciences, 231141)
Phosphate buffered saline (“PBS”)
Test compounds gold nanocrystal formulations GT033 and GD-007.
Vehicle: Water.
Treatment Groups and Dosages
[0801] Control Group 1, First Treatment “Group 2” and Second Treatment “Group 3” each had 10 animals per group.
Group 1: Day 0 CII/CFA, given normal drinking water from day 0-42.
Group 2: Day 0 CII/CFA, gold nanocrystal formulation (GT033; Example 4/Table 1d; gold ppm 2.0) as drinking water from day 0-42.
[0802] Group 3: Day 0 CII/CFA, gold nanocrystal formulation (GD-007; Example 5/Table 2a; gold ppm 14.8) as the only liquid for drinking from day 0-42.
Protocol
[0803] 1. On arrival of animals, the health of all animals was checked and after passing the health test, each was numbered with a unique ear tag. [0804] 2. The animals were allowed to acclimate for at least 72 hours. [0805] 3. Chicken Type II collagen was prepared so as to achieve a suspension with a concentration of about 16 mg/ml in 0.1M acetic acid. After dissolution overnight at 4° C., the solution was diluted with cold PBS to achieve a suspension with a concentration of about 8 mg/ml. [0806] 4. Fresh mycobacterium was prepared by grinding it finely with a mortar and pestle and adding about 7 ml of IFA, drop-by-drop, to create an emulsion or suspension of CFA with a final concentration of about 5 mg/ml. [0807] 5. An emulsion of Chicken Type II collagen and CFA was prepared using approximately equal volumes of each to result in the injectable suspension of collagen in CFA (i.e., “CII/CFA”). [0808] 6. On Day 0, the animals were injected with 50 μl of the CII/CFA solution at the base of the tail. [0809] 7. Treatments using gold nanocrystal formulation GT033 (i.e., Group 2) and gold nanocrystal formulation GD-007 (i.e., Group 3) were given according to the schedule above until Day 42. Specifically, each water bottle containing either normal drinking water, GT033 or GD-007 was topped-off as needed either every other day or every third day. The bottles were not specifically cleaned or specifically emptied during the 42-day trial. [0810] 8. The limb scores were determined three times per week from Day 14 to the end of the study. Each of the four limbs was given a score according to the following; [0811] 0=Normal. [0812] 1=Slight swelling of whole joint or individual digit inflammation. [0813] 2=Intermediate swelling of whole joint with redness and/or inflammation in more than one digit. [0814] 3=severe joint inflammation and redness spreading to multiple digits. [0815] 4=severe joint inflammation and redness spreading to multiple digits; overt signs of bone remodeling. [0816] 9. All animals were bled on days 0 and day 42 and the retrieved serum was stored for optional analysis. [0817] 10. The animals were sacrificed on Day 42 and the ankle joints were removed and placed in neutral-buffered formalin in preparation for histopathology. [0818] 11. These sections were processed and stained with hematoxylin and eosin stain (“H & E”) and were scored by a qualified (and experimentally blinded) histopathologist using a semi-quantitative measurement of the degree of infiltration and damage.
[0819]
[0820] Histopathology was performed on the left and right paws from each of the 10 mice in Group 1 (control) and Group 3 (GD-007). No histopathology was performed on Group 2 mice.
[0821] Each pair of paws was assigned a Pathology numerical code (e.g., R0248-09 for one mouse in Group 1) and the limbs distinguished as left (“L”) or right (“R”) from each numbered animal.
Histopathology/Methodology:
[0822] The skin was dissected from the paw. [0823] The dissected samples were decalcified to permit sectioning. [0824] The decalcified samples were routinely processed, sectioned and one H & E-stained section was prepared for examination. This included both halves of each specimen being hemi-sectioned. [0825] Each histopath paw was scored as described below. Samples were scored in blinded fashion, without knowledge of the experimental protocol or identity of groups. [0826] Multiple phalangeal and tarsal joints were generally present on each section. Scoring related to the most severely affected of these joints in each case.
Scoring System
[0827] In this instance, three aspects of the joint pathology were scored individually to contribute to a composite score (i.e., maximum possible score=9). Thus, the higher the number, the greater the damage. Representative photomicrographs of joints corresponding to the aforementioned grades 0-3 are shown in
TABLE-US-00030 TABLE 15 Aspect Grade 0 Grade 1 Grade 2 Grade 3 Inflammation Normal joint Mild synovial Synovial hyperplasia Synovial hyperplasia hyperplasia with with moderate to with marked inflammation inflammation marked inflammation involving both neutro- dominated by involving both phils and macrophages. neutrophils. Low neutrophils and Loss of synoviocyte lining. numbers of macrophages. Inflammation may extend neutrophils and Neutrophils and from synovium to macrophages in macrophages in surrounding tissue joint space. joint space; may be including muscle. some necrotic tissue Numerous neutrophils and debris. macrophages in joint space, together with significant necrotic tissue debris. Articular cartilage Normal joint Articular cartilage Articular cartilage Significant disruption damage shows only mild shows moderate and loss of articular degenerative change. degenerative change cartilage with extensive Early pannus formation and focal loss. Pannus pannus formation. may be present formation is present peripherally. focally. Damage to Normal joint No change to May be focal Disruption or collapse underlying underlying necrosis or fibrosis of metaphyseal bone. metaphyseal metaphyseal bone. of metaphyseal Extensive inflammation, bone bone. necrosis or fibrosis extending to medullary space of the metaphysis.
TABLE-US-00031 TABLE 16 Paw Histopathology Scoring Mouse Pathology Number Total Number and Limb Inflammation Cartilage Bone score Comments Control R0248-09 1.1 L 1 0 0 1 Few neutrophils in mildly thickened synovium ideally. 1.1 R 2 2 2 6 R0249-09 1.2 L 3 2 2 7 1.2 R 1 0 0 1 R0250-09 1.3 L 3 2 2 7 1.3 R 0 0 0 0 R0251-09 1.4 L 3 2 2 7 1.4 R 3 1 1 5 Reaction localized to P1-metatarsal R0252-09 1.5 L 3 2 2 7 1.5 R 3 2 2 7 R0253-09 1.6 L 0 0 0 0 1.6 R 3 1 2 6 R0254-09 1.7 L 3 2 2 7 1.7 R 3 2 2 7 R0255-09 1.8 L 0 0 0 0 1.8 R 3 1 1 5 R0256-09 1.9 L 0 0 0 0 1.9 R 0 0 0 0 R0257-09 1.10 L 0 0 0 0 1.10 R 0 0 0 0 Treatment R0258-09 2.1 L 0 0 0 0 Group3 2.1 R 0 0 0 0 R0259-09 2.2 L 0 0 0 0 2.2 R 0 0 0 0 R0260-09 2.3 L 0 0 0 0 2.3 R 0 0 0 0 R0261-09 2.4 L 0 0 0 0 2.4 R 0 0 0 0 R0262-09 2.5 L 0 0 0 0 2.5 R 0 0 0 0 Has localized subcutaneous inflammatory response; joints normal. R0263-09 2.6 L 0 0 0 0 2.6 R 0 0 0 0 R0264-09 2.7 L 0 0 0 0 2.7 R 0 0 0 0 R0265-09 2.8 L 0 0 0 0 2.8 R 0 0 0 0 R0266-09 2.9 L 3 1 0 4 2.9 R 0 0 0 0 R0267-09 2.10 L 3 1 2 6 Localized metatarsal-P1 reaction with marked periosteal new bone and cartilage formation - probably localized fracture repair rather than joint disease. 2.10 R 3 2 2 7
TABLE-US-00032 TABLE 17 Mean Group Scores Number [%] of Group Paws (n=) Mean Score Joints affected 1-Control 20 3.65 14/20 [70%] 2-GD-007 20 0.85 3/20 [15%]
[0828] As is typical for this type of murine CIA model, one animal in Treatment “Group 3,” GD-007, (i.e., R0266-09) exhibited a lack of correlation between its right and left joints in terms of the presence/absence of arthritis. Similar discrepancies occur in some of the control mice, as well as differences in the severity of the arthritis between different joints in the same mouse (e.g., R0250-09).
[0829] It is clear, however, that the most severe pathology occurred in Control Group 1 (i.e., drinking water) and the least severe pathology occurred in First “Treatment Group 2” (i.e., gold nanocrystal formulation GD-007).
[0830] One animal in Treatment Group 3 (i.e., R0267-09) suffered a broken bone which probably accounted for its higher scores. Exclusion of this animal resulted in a mean score of 0.22. Further, the histopathology data suggests no resulting damage at all in 8 of the 10 mice (i.e., 16 total paw joints examined). Clearly the gold nanocrystal formulation GD-007 had a significant positive effect in this CIA test.
[0831] It is clear that the gold nanocrystal formulations produced according to the invention significantly reduced the negative induced arthritis effects in the CIA model, relative to the control. It is known that reduction of excessive IL-6 and/or reduction of excessive MIF both reduce the negative effects of arthritic conditions. Accordingly, without wishing to be bound by any particular theory or explanation, by reducing excessive MIF, and/or one or more signaling pathways associated with MIF, arthritic conditions can be reduced. The gold nanocrystalline formulation GD-007 showed significantly improved results, relative to the control. These results, along with the results shown in the in vitro example and the EAE mouse model Example herein, suggest that the inventive gold nanocrystal compositions may be altering MIF and/or more signaling pathways associated with MIF, as well as IL-6.
Example: Doses Comparison
[0832] As stated above, in the gold nanocrystal trial, each mouse had access to GD-007 solution as the only source of drinking fluid. To calculate the dose of gold consumed by a mouse per day, following equation was used:
Dose=Volume consumed (ml)×Concentration (mg/L) Animal weight (kg)
[0833] where [0834] Dose is the nanocrystal gold consumed per mouse per day in mg/kg/day, [0835] Volume is an average amount of GB-134 solution drunk by a mouse per day in mL/day, [0836] Concentration is the amount of nanocrystal gold in the GD-007 solution in mg/mL, [0837] Weight is a mouse body weight in kg.
[0838] The following assumptions were used to calculate the nanocrystal gold dose: [0839] Volume=4 mL [0840] Concentration=0.0148 mg/mL [0841] Weight=0.025 kg
[0842] This results in a nanocrystal gold dose of 2.4 mg/kg/day.
[0843] Below is the comparison of the gold content in doses typically used for Auranofin treatment in the type II collagen-induced arthritis mouse model. Typical Auranofin dose is 40 mg/kg/day (Agata et al., 2000). Since the gold content in Auranofin is 29%, this results in gold dose of approximately 12 mg/kg/day.
[0844] In the only known human study (Abraham et al. 1997, 2008) using gold nanoparticles, a 30 mg/day gold nanoparticle dose was used for patients weighing from 108 to 280 lb. This corresponds to approximately 0.24 to 0.61 mg/kg/day gold nanoparticle dose.
[0845] A comparison between dose levels of gold content in Auranofin, gold in gold nanoparticles, and the novel gold nanocrystals, used in these different efficacy studies, is shown below in Table 17a, demonstrating that the present novel gold nanocrystals are fundamentally different from, and perform very differently and at a much higher level of potency than, conventional gold, whether in molecular form in Auranofin, or in nanoparticle form as in Abraham, et. al.
TABLE-US-00033 TABLE 17a Study Type of Gold Product Gold mg/kg/day Mouse RA CIA Novel Gold Nanocrystals 2.4 Agata/Mouse RA CIA Auranofin 12 (5X) Estimated Human dose* Novel gold Nanocrystals 0.005 Abraham/human Colloidal gold 0.24 to 0.61 (47X to 122X) *Using mouse/mouse Auranofin/Nanocrystals potency factor applied to Auranofin human dose
Example 26
Acute Murine Model of Experimental Auto-Immune Encephalitis (“EAE”)
Summary
[0846] This Example demonstrates the efficacy of the inventive gold nanocrystalline composition GB-056 in a mouse EAE model. Female Biozzi mice 7-8 weeks old were challenged in the flank with mouse spinal cord homogenate in CFA on day 0 of the study by injection at the base of the tail. Ten treatment group mice were orally administered the gold nanoparticle suspension treatment GB-056 (i.e., as discussed in Example 17) as their only liquid for drinking by using standard water bottles. Fresh gold nanocrystalline formulation GB-056 was provided daily along with clean water bottles. Control group mice were provided ordinary tap drinking water. Clinical scoring in this EAE test was completed by a standard scoring system of 0-5.0 scored from day 1 until termination at day 28. Those results are presented in Tables 9a and 9b, as well as in
Methodology
Animals
[0847] Species: Mice [0848] Strain: BIOZZI [0849] Source: Harlan [0850] Gender and number: Female, 20 [0851] Age: About 7-8 weeks old at the start of the study. [0852] Identification: Each mouse was given a unique identity number. [0853] Animal husbandry: On receipt, all animals were examined for external signs of ill-health and all unhealthy animals were excluded from further evaluation. Animals were housed in groups of five under specific pathogen free (spf) conditions, in a thermostatically monitored room (22±4° C.) in an animal unit. Animals were equilibrated under standard animal house conditions for at least 72 hours prior to use. The health status of the animals was monitored throughout this period and the suitability of each animal for experimental use was assessed prior to study start. [0854] Housing Animals were housed in groups of 10 per cage in a controlled room, to ensure correct temperature, humidity and 12-hour light/dark cycle for the duration of the study. [0855] Diet: Irradiated pellet diet and water was available ad libitum throughout the holding, acclimatization and post-dose periods.
Compound and Reagents
[0856] Mouse and Spinal Cord Homeogenate (“MSCH”) produced in-house.
Incomplete Freund's Adjuvant (“IFA”) (Sigma, FF5506)
[0857] Mycobacterium tuberculosis H37Ra (BD Biosciences, 231141)
Phosphate buffered saline (“PBS”) in-house.
Test compound gold nanocrystalline suspension GB-056 (discussed elsewhere herein)
Vehicle: Water.
[0858] Treatment Groups and Dosages
Control Group 1 and the Treatment Group 2 each had 10 animals per group.
Group 1: Day 0 a mixture of MSCH/IFA/tuberculosis (see Protocol below) was injected into each mouse at base of tail and each was given normal drinking water dispensed from a water bottle, from day 0 to day 28.
Group 2: Day 0 a mixture of MSCH/CFA/tuberculosis was injected into each mouse at base of tail and each was given gold nanocrystal formulation (GB-056) dispensed from a daily-cleaned water bottle with fresh GB-056 provided daily, as the only liquid for drinking, from day 0 to day 28.
Protocol
[0859] On arrival of animals, the health of all animals was checked and after passing the health test, each was numbered with a unique ear tag. [0860] 1. The animals were allowed to acclimate for at least 72 hours. [0861] 2. The spinal cord was reconstituted in PBS containing Mycobacterium tuberculosis H37RA. This resulted in 6.6 mg/ml of MSCH and 400 ug/ml of H37RA. An equal volume of Freund's incomplete adjuvant was added to this mixture to make the final immunogen (3.3 mg/ml SCH and 200 ug/ml H37RA). This mixture could not be considered complete Freund's because amount of mycobacterium was much lower. [0862] 3. On Day 0, the animals were injected with 50 μl of the solution discussed in step 3 at the base of the tail. [0863] 4. Treatment using gold nanocrystal formulation GB-056 was given according to the schedule above until Day 28. Fresh GB-056 was provided daily (i.e., replaced approximately every 24 hours). [0864] 5. The scores were determined daily from Day 1 to the end of the study. Scoring of each mouse occurred according to the following; [0865] 0: Normal [0866] 0.5: Paretic tail [0867] 1.0: Flaccid tail [0868] 1.5: Slow and/or absent righting reflex [0869] 2.0: One hind limb paralysis [0870] 2.5: One hind limb paralysis and unusual gait [0871] 3.0: Two hind limbs paralysis [0872] 3.5: Two hind limbs paralysis+one front limb paresis [0873] 4.0: Two hind limbs paralysis+one or two front limb paralysis [0874] 5.0: Moribund [0875] 6. The animals were sacrificed on Day 28 and the brain and spinal cord were removed and placed in neutral-buffered formalin in preparation for histopathology. [0876] 7. These sections were processed and stained with hematoxylin and eosin stain (“H & E”). Tables 9a and 9b show the raw scoring for each of the 20 mice in this EAE study.
TABLE-US-00034 TABLE 18a Animal Day Day Day Day Day Day Day Day Day Day Day Day Day Day Day Day Day Day Day # 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 Water Control 1 0 0 0 0 0 0 0 0 0 0 1.5 2 2.5 5 5 5 5 5 5 2 0 0 0 0 0 0 0 1.5 1.5 1.5 2.5 2.5 5 5 5 5 5 5 5 3 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 1.5 1.5 1.5 0 4 0 0 0 0 0 0 0 1 1 2.5 1.5 1.5 1.5 1.5 1.5 1.5 1.5 1.5 0 5 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 1.5 6 0 0 0 0 0 0 0 0 1.5 1.5 1.5 5 5 5 5 5 5 5 5 7 0 0 0 0 0 0 0 0 0 0 1.5 2 2.5 1.5 1.5 1.5 1.5 1.5 0 8* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 9 0 0 0 0 0 0 0 0 0 1 1.5 2 2 2 2 2 1.5 1.5 0 10 0 0 0 0 0 0 0 0 0 0 0 1.5 1.5 3 3 3 3 3 3 GR-056 1 0 0 0 0 0 0 0 0 0 0 0 0 0 0 1.5 1.5 2.5 3 3 2 0 0 0 0 0 0 0 0 0 0 0 1.5 2 2.5 3 3 2.5 1.5 1.5 3* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 4 0 0 0 0 0 0 0 0 0 1.5 1.5 2 5 5 5 5 5 5 5 5* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 6* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 7* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 8* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 9* 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 10 0 0 0 0 0 0 0 0 0 1 1.5 1.5 1.5 1.5 1.5 2.5 3 3 1.5 *= Disease Free
TABLE-US-00035 TABLE 18b Day Day Day Day Day Day Day Day Day Day 10 11 12 13 14 15 16 17 18 19 MEAN Water Control 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.25 0.40 0.65 GR-056 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.25 SEM Water Control 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.17 0.21 0.29 GR-056 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.00 0.17 INCIDENCE Water Control 0 0 0 0 0 0 0 20 30 40 GR-056 0 0 0 0 0 0 0 0 0 20 CUM. INCIDENCE Water Control 0 0 0 0 0 0 0 20 30 40 GR-056 0 0 0 0 0 0 0 0 0 20 CUM. DISEASE FREE Water Control 100 100 100 100 100 100 100 80 70 60 GR-056 100 100 100 100 100 100 100 100 100 80 Day Day Day Day Day Day Day Day Day 20 21 22 23 24 25 26 27 28 MEAN Water Control 1.00 1.65 2.00 2.30 2.30 2.45 2.40 2.40 1.95 GR-056 0.30 0.50 0.85 0.90 1.10 1.20 1.30 1.25 1.10 SEM Water Control 0.29 0.48 0.59 0.66 0.66 0.62 0.63 0.63 0.73 GR-056 0.20 0.26 0.52 0.53 0.54 0.56 0.57 0.57 0.54 INCIDENCE Water Control 60 70 70 70 70 80 80 80 50 GR-056 20 30 30 30 40 40 40 40 40 CUM. INCIDENCE Water Control 60 70 70 70 70 80 80 80 90 GR-056 20 30 30 30 40 40 40 40 40 CUM. DISEASE FREE Water Control 40 30 30 30 30 20 20 20 10 GR-056 80 70 70 70 60 60 60 60 60
[0877]
[0878]
[0879] As is typical for this EAE model, one animal in Treatment Group 2 (i.e., animal 4) died; whereas 3 animals in Control Group 1 died.
[0880] The most severe pathology occurred in Control Group 1 and the least severe in Treatment Group 2.
[0881] The one animal in Treatment Group 2 that died (i.e., animal 4) caused the group to have a much higher score. Clearly the inventive gold nanocrystal suspension GB-056 had a significant positive effect in this EAE test. Without wishing to be bound by any particular theory or explanation, the results of this Example, in combination with the results of the murine CIA model and the in vitro MIF cytokine analysis, strongly suggest that MIF, and/or MIF signaling pathways, are being favorably influenced by the inventive gold nanocrystalline compositions of the present invention.
Example 27
Long Term Exposure of Gold Nanocrystal Suspension GD-013 in Mice
[0882] The purpose of this Example was to observe if any negative toxicology effects occurred in mice when the mice drank, ad libitum, gold nanocrystal suspension GD-013 as their only source of liquid for an extended period of time.
[0883] A total of 25 female mice were used in this Example, five (5) in the control group; and ten (10) in each of two treatment groups. The control group received regular bottled water in their drinking bottles. The two treatment groups received two different concentrations of GD-013 as their only drinking liquid. A first treatment group received a 50% GD-013 crystal suspension (with the other 50% being purified DI/RO water) while the second treatment group received 100% GD-013 crystal suspension. All groups were permitted to drink as much, or as little, as desired; food was provided ad libitum as well. The weight of each animal and the average amount of liquid consumed were recorded weekly. At week 23 of the study, 6 mice were sacrificed (3 mice from each of the GD-013 crystal suspension treatment groups) for necropsy and pathology. The remaining mice continued to consume the two treatment suspensions through 46 weeks.
Materials and Methods:
[0884] In this type of exposure study it is acceptable to use only one sex, females, for the purposes of testing for toxicity. Data from other studies have shown that there is generally no difference between the sexes, but when one sex does react more strongly it is typically the females. Males are only used when there is some form of evidence indicating that they may have a stronger reaction. Since, there is no such information indicating that males would be affected in this way, only females were used. The females used were adult, nulliparous and non-pregnant. The Swiss Webster strain of outbred mice was used in this example. This strain was chosen because of its widespread use in general purpose and toxicology research. It also is known to not have any detrimental genetic deficits that could potentially interfere with data collection.
TABLE-US-00036 TABLE 19 Study Information Mode of Adminis- Species Strain Group tration Doses Duration Mus Swiss Control - 5/F Via Water Ad 23 weeks musculus Webster 50% GD-013 - Bottle libitum and 46 10/F weeks 100% GD-013 - 10/F
Dose Preparation
[0885] All treatment groups involved in this study received the referenced GD-013 nanocrystalline suspensions in their water bottles. The mice were allowed to drink free choice. The control group received purified, bottled water.
TABLE-US-00037 TABLE 20 GD-013 Treatment Information Treatment Group Lot Numbers Au Content Control Bottled Water 0.0 ppm Au 50% GD-013 Au 50/50 GD-013/RO H.sub.2O 7.6 ppm Au 50% RO H.sub.2O 100% GD-013 Au GD-013 15.2 ppm Au
Housing and Feeding
[0886] All study personnel entering the mouse study area wore personal protection clothing (i.e. gloves, face mask, and shoe covers). Mice were purchased from Harlan Laboratories. Upon receipt of the mice, the mice were given permanent identification in the form of a tail tattoo (Harvard Apparatus Tattoo). The mice were then randomly assigned and housed by groups of 5 mice per cage. The cages were large enough to allow adequate room for 5 individuals and were not so small as to hinder clear observations of each animal. The mice were acclimated to the lab environment for a period of one week. The housing area was maintained at a constant temperature of 22° C. (f 3° C.), and the relative humidity was maintained at 30%-50%. Artificial, full spectrum lighting was used (PureLite 60 w, 120 v bulbs). Timers were used to achieve a 12-hour light 12-hour dark cycle. Food was provided ad libitum (Purina Certified Rodent Diet 5002). Standard corncob bedding was provided in the cages. Cage changes were carried out once weekly. When an animal was found dead the cage that it was housed in was changed immediately after the dead animal was removed.
Procedure and Observation
[0887] After the acclimation period, both treatment groups began receiving the noted GD-013 nanocrystalline suspensions in their water bottles. The control group continued to receive purified drinking water. On the first day of treatment each mouse was weighed, and their weights were recorded. At the start of each week, all of the mice were again weighed, and their weights recorded. Also, the approximate amount of water and GD-013 crystal suspension consumed, was recorded each week. Throughout the study the mice were observed for any abnormalities or signs of distress.
Weight Gain
[0888] When the study began, all of the mice were approximately the same weight. Each week, each animal was weighed, and its weight was recorded. The individual weights of each animal in the groups were then averaged and plotted graphically in
Average Daily Consumption
[0889] Every week the amount of: (1) water, (2) 50% GD-013, and (3) 100% GD-013 that each group consumed was measured. Once the amount of liquid, 50% purified water, that had been consumed during the previous week had been determined, calculations were made to find an approximate daily intake per animal over the course of the week. The liquid consumption data for 46 weeks is shown in
Results/Conclusions:
Weight Gain
[0890] Statistical analysis of the average weights of the groups was performed to determine if there was any difference in weight gain and/or loss between the groups. Each treatment group was compared to the control group; and the two treatment groups were also compared to each other. Overall there was a statistically significant weight loss between the 100% GD-013 Treatment Group and the Control Group (P<0.05). There was no statistically significant weight gain/loss between the two Treatment Groups or between the 50% GD-013 Treatment Group and the Control Group.
Average Weekly Consumption
[0891] All three of the groups consumed what is considered to be normal amounts of liquid daily, so dehydration was not an issue. Again, statistical analyses of the consumption values for each group was performed to determine if there was a significant difference in consumption. Both Treatment Groups were compared to the Control Group and both Treatment Groups were compared to each other. The Control Group consumed significantly less than both Treatment Groups (P<0.05). There was no statistical difference between the amounts consumed by the Treatment Groups (P>0.05). There were no observable differences in health, behavior, or issues related to dehydration.
Mortality
[0892] There were two recorded deaths in the study, one from each Treatment Group. The first death occurred in the 50% GD-013 group at week 20. The second death occurred at week 22 in the 100% GD-013 group. The mouse from the 50% GD-013 treatment group had always been much smaller than the rest and had not been gaining weight; the cause of this is unknown. The other mouse had not shown any indicators of distress or poor health. No pathology was possible for these two mice.
Pathology
[0893] Three mice from each treatment group were submitted for pathology at week 23. The following organs were submitted for histopathological evaluation: heart, thymus, lung, liver, kidney, spleen, stomach, duodenum, jejunum, ileum, cecum, colon, urinary bladder, ovary, striated muscle, haired skin, bone marrow (femur/tibia), pituitary and brain. The pathology findings concluded that despite some of the abnormalities that were noted, all were considered incidental findings that were associated with normal variation between individuals and normal wear and tear. None of the findings in the pathology report indicated any degree of toxicity to target organs. The pathologist was completely blind to what treatment the mice in the study received, nor did the pathologist have any knowledge of treatment in control mice in order to eliminate possible bias in the pathology findings.
[0894] All tissues referenced above were grossly examined and only the spleen and liver were found to have minimal to mild variations in color. The only specific histopathological findings are reported in Table 21. The numbers “2-3,” “2-5” and “4-7” in the 50% GD-013 row refer to three different mice, to which the “Comments” are directed. Likewise, the histopathology “Comments” regarding the spleen are directed to three mice, “3-3,” “5-9” and “5-10;” whereas the “Comments” regarding the liver apply to only one mouse (i.e., “5-10”). All gross examinations were consistent with congestion from euthanasia and/or fat storage and were considered to be within normal limits. No gross lesions were noted.
TABLE-US-00038 TABLE 21 Pathology Findings Histopathological Group Findings Comments 50% Spleen: Hematopoiesis, EMH: normally observed in GD-013 extramedullary, multifocal, minimal to moderate minimal red pulp (2-3, 2-5, degrees; is considered a 4-7 common, incidental finding not indicative of toxic change or infection 100% Spleen: Hematopoiesis, EMH: normally observed in GD-013 extramedullary, multifocal, minimal to moderate minimal to moderate, red degrees; is considered a pulp (3-3, 5-9, 5-10) common, incidental finding Liver: Microgranuloma, not indicative of toxic focal, minimal, hepatocytes change or infection (5-10 Liver: Condition considered to be from bacterial showering from the hepatic portal system; not indicative of infection or toxic change
Example 28
35-Day Uptake and Distribution Acute Toxicity Study
[0895] The purpose of this 35-day study was to determine the uptake and distribution and acute toxicity (if any) of two crystal suspensions (GB-134 and GB-151) and compare the results to a commercially available Mesogold product. Thirteen mice were involved in this study. Concentrations of gold were determined in the urine and the feces, as well as in certain vital organs and blood of the test animals. Additionally, a selection of organs from some individuals were examined histologically to determine if there were any abnormalities. Further, all mice were permitted to drink up to the point that they were sacrificed for this study. This procedure was followed to insure, for example, that accurate gold concentrations in the blood could be determined.
Materials and Methods:
[0896]
TABLE-US-00039 TABLE 22 Study Information Mode of Adminis- Species Strain Group tration Doses Duration Mus Swiss Mesogold - Free Mesogold, 35 days musculus Webster 3/F Choice GB-134, GB-134 - GB-151 10/F GB-151 - 10/F
Dose Preparation
[0897] All treatment groups involved in this study received their solutions in their water bottles. The mice were allowed to drink free choice. Each group received either: (1) Mesogold, (2) GB-134, or (3) GB-151 (all of which were not diluted) in their drinking bottles.
TABLE-US-00040 TABLE 23 Au Solution Treatment Information Treatment Group Lot Numbers Au Content Mesogold Mesogold 19.8 ppm Au GB-134 GB-134 8.9 ppm Au GB-151 GB-151 8.3 ppm Au
Procedure and Observation
[0898] After the animals received their respective treatments for one day, metabolic cage collections of urine and feces were initiated. A total of nine animals per week were housed in the metabolic cages and had their urine and feces collected. While in the metabolic cages the subject mice continued to receive in their water bottles the liquid they had been assigned to drink. The amount of liquid consumed during the 24-hour period was also measured and recorded. The urine and feces samples were then collected and tested for Au concentration. The volume of urine excreted, and the weight of feces collected were also measured and recorded.
[0899] At the end of the study, all 13 animals were sent to Taconic Laboratories (Rockville, Md.) for the performance of a gross necropsy and pathology report or to have organ and blood samples collected and returned for further analysis (discussed later herein). Microscopic evaluations were performed on the following tissues: heart, lung, liver, spleen, kidney, brain, stomach, duodenum, jejunum, ileum, cecum and colon. Additionally, certain heart, lung (left and right), liver, spleen, kidney (left and right), and brain were collected and returned in an empty, sterile glass vial for further concentration analysis.
Procedure for the Digestion of Feces and Urine Samples
[0900] Specific methods were developed to determine the amount of gold in the feces and the urine. PTFE sample cups and microwave digestion bombs were ordered from Fisher Scientific and obtained from Parr Instrument Company). 23 mL PTFE sample cup (Fisher Cat No. 0102322A) and Parr 4781 microwave digestion bomb (Fisher Cat No. 0473155) were used for digestion.
[0901] The microwave used was a Panasonic 1300 Watt. Model No. NN-SN667 W, Serial No. 6B78090247.
Urine
[0902] 1.5 grams of urine was weighed in a PTFE sample cup. When urine exceeded that mass, another digestion was prepared. When the urine sample mass was below 1.5 grams the appropriate amount of D.I. water was added to bring the mass up to approximately 1.5 grams. 0.24 mL of 50% v/v HNO.sub.3 was added to the sample cup, followed by 0.48 mL of 36% v/v HCl. The sample cup was sealed and placed inside a microwave bomb. The microwave bomb was sealed and placed in the center of a microwave. The sample was irradiated until the Teflon indicator screw raised up 1 mm from the top of the bomb. The time the bomb spent in the microwave ranged between 30 to 60 seconds depending on the urine sample. The microwave digestion bomb was removed from the microwave and cooled for 20-30 minutes, until the Teflon indicator screw was lowered to its original position. The sample cup was removed from the microwave digestion bomb, and the liquid sample was transferred to a vial for testing.
Feces (1 Pellet Sample):
[0903] A singe fecal pellet was weighed in a PTFE sample cup. 5 mL of D.I. water was added to the sample cup. 0.8 mL of 50% v/v HNO.sub.3 was added to the sample cup, followed by 1.6 mL of 36% v/v HCl. The sample cup was sealed and placed inside a microwave bomb. The microwave bomb was sealed and placed in the center of the microwave. The sample was irradiated until the Teflon indicator screw raised up 1 mm from the top of the bomb. The time the bomb spent in the microwave ranged between 20 to 30 seconds depending on the mass of the 1 pellet fecal sample. The microwave digestion bomb was removed from the microwave and cooled for 20-30 minutes, until the Teflon indicator screw was lowered to its original position. The sample cup was removed from the microwave digestion bomb, and the liquid sample was transferred to a vial for testing.
Bulk Feces Sample
[0904] About 0.300 grams of feces was weighed in a PTFE sample cup. 5 mL of D.I. water was added to the sample cup. 0.8 mL of 50% v/v HNO.sub.3 was added to the sample cup, followed by 1.6 mL of 36% v/v HCl. The sample cup was sealed and placed inside a microwave bomb. The microwave bomb was sealed and placed in the center of a microwave. The sample was irradiated until the Teflon indicator screw raised up 1 mm from the top of the bomb. The time the bomb spent in the microwave ranged between 20 to 40 seconds depending on the mass of the bulk feces sample. The microwave digestion bomb was removed from the microwave and cooled for 20-30 minutes, until the Teflon indicator screw was lowered to its original position. The sample cup was removed from the microwave digestion bomb, and the liquid sample was transferred to a vial for testing. Bulk feces samples may require several digestions to digest all the feces present in the original sample.
Note: If the sample didn't appear to be fully digested (i.e. solids still present/discoloration on the PTFE sample cup's side walls) a second digestion was performed. This required a second addition of the volumes of D.I. water, 50% v/v HNO.sub.3 and 36% v/v HCl specified for the appropriate sample. (See above procedures for correct volumes) The sample was then microwaved again, and allowed to cool for 20-30 minutes before transferring to a sample vial for testing.
*D.I. water=Deionized water.
*PTFE=polytetrafluoroethylene
[0905] One digested, all samples were analyzed using the atomic absorption spectroscopy techniques discussed above herein.
[0906] The pathology findings for the 35-day study are shown in Table 24. All tissues were grossly examined and only the spleen and liver were found to have minimal to mild variations in color. All gross examinations were consistent with congestion from euthanasia and/or fat storage and were considered to be within normal limits. No gross lesions were noted. The comments were directed to specific mice and are noted in Table 24. The designation “M-3” refers to one mouse in the Mesogold group; whereas “GB-134-7” refers to one mouse in the “GB-134” group; and “G151-9” refers to one mouse in the “GB-151” group.
TABLE-US-00041 TABLE 24 Histopathological Group Findings Comments Mesogold Spleen: Hematopoiesis, EMH: normally observed in extramedullary, multifocal, minimal to moderate minimal to moderate, red degrees; is considered a pulp (M-3) common, incidental finding Liver: Microgranuloma, not indicative of toxic focal, minimal, hepatocytes change or infection (M-3) Liver: Condition considered to be from bacterial showering from the hepatic portal system; not indicative of infection or toxic change GB-134 Spleen: Hematopoiesis, EMH: normally observed in extramedullary, multifocal, minimal to moderate minimal red pulp (GB-134- degrees; is considered a 7, GB-134-8) common, incidental finding Liver: Microgranuloma, not indicative of toxic focal, minimal, hepatocytes change or infection (GB-134-8) Liver: Condition considered to be from bacterial showering from the hepatic portal system; not indicative of infection or toxic change GB-151 Spleen: Hematopoiesis, EMH: normally observed in extramedullary, multifocal, minimal to moderate minimal to moderate, red degrees; is considered a pulp (GB-151-9, GB-151- common, incidental finding 10) not indicative of toxic change or infection
[0907]
[0908]
[0909]
TABLE-US-00042 TABLE 25 Average Weekly Amount of Au Found in Feces Treatment Groups Week Meso (ppm) GB-134 (ppm) GB-151 (ppm) 0 1.7286 0.5343 0.6871 1 58.8611 24.3989 24.8668 2 59.0330 19.1658 27.4792 3 91.3662 15.9090 19.6045 4 86.5076 18.4982 18.1742 5 65.3942 20.3575 24.9802
[0910]
TABLE-US-00043 TABLE 26 Average Weekly Amount of Au Found in Urine Treatment Groups Week Meso (ppm) GB-134 (ppm) GB-151 (ppm) 0 0.0090 0.0240 0.0330 1 0.1318 0.0821 0.0263 2 0.1004 0.3453 0.0727 3 0.4471 0.1518 0.1264 4 0.1457 0.0920 0.0360 5 0.1953 0.0261 0.0380
Procedure for Neutron Activation Analysis Measurements of Tissue Samples and Blood
[0911] Certain samples of heart, liver, spleen, kidney, brain and blood were analyzed for gold content. Specifically, neutron activation analysis was utilized. Instrumental neutron activation analysis (NAA) is especially powerful in its sensitivity and its ability to determine accurately many elements in a single sample. NAA does not require any chemical treatments or special chemical preparation of samples, thus minimizing the possibilities of losses, contamination and any incomplete tissue sample dissolution, for example.
[0912] The NAA method involves weighing the tissue sample in polyethylene vials. An inert material is added to each vial to prevent evaporative loss. Each vial is uniquely identified with a bar code and a neutron flux monitor affixed to the base of each vial. These vials are stacked into one-foot long bundles for irradiation with neutrons from a nuclear reactor. The bundles contain randomly selected duplicate samples and gold standards (or known concentrations of gold) are inserted at random positions in the bundles.
[0913] All bundles are treated in a similar manner. The bundles are submitted for exposure to a flux of neutrons at a nuclear reactor. Specifically, the bundles are inserted into the core of a nuclear reactor for about 45 minutes. The bundles are rotated during irradiation so that there is no horizontal flux variation. (The vertical flux variation is monitored with the individual flux monitors.) This irradiation causes any gold present in the sample to become radioactive and gold then begins to emit radiation in the form of penetrating gamma rays whose energies (or wavelengths) are characteristic of gold (e.g., Au 198, 411.8 keV).
[0914] After a decay period of about six days, the irradiated samples are loaded onto a counting system. Specifically, each radiated and partially decayed sample is placed adjacent to a gamma-ray spectrometer with a high resolution, coaxial germanium detector. Gamma rays radiate continuously from each sample (so long as gold is present) and the interaction of the radiated gamma rays with the detector leads to discrete voltage pulses proportional in height to the incident gamma-ray energies. A specially developed multi-channel analyser sorts out the voltage pulses from the detector according to their size and digitally constructs a spectrum of gamma-ray energies versus intensities. The counting time is about 45 minutes per sample. By comparing spectral peak positions and areas with library standards, gold is both qualitatively and quantitatively identified. The results of the analysis are set forth below.
[0915] In conjunction with Table 27 below,
[0916] Gold was not detected in two brain samples, GB-151-6 and GB-134-3, with the detection limit of 0.35 ppb and 0.25 ppb, respectively. Blood samples GB-151-5 and GB-134-3 were not analyzed because of insufficient amount available for analysis.
TABLE-US-00044 TABLE 27 Gold concentration in different tissue samples and blood measured by NAA. Sample ID Sample mass, g Gold wt %, ppb GB-151-4, -5 Heart* 0.356 0.89 ± 0.187 GB-151-5 Liver 1.536 1.76 ± 0.107 GB-151-4, -5 Spleen* 0.213 1.74 ± 0.244 GB-151-4, -5, -5 Kidney* 0.661 2.54 ± 0.170 GB-151-4, -5 Brain* 0.889 0.73 ± 0.102 GB-151-6 Heart 0.129 0.94 ± 0.329 GB-151-6 Liver 0.899 2.34 ± 0.140 GB-151-6 Spleen 0.093 4.00 ± 0.480 GB-151-6 Blood 0.386 1.06 ± 0.212 GB-151-6 R& L Kidney 0.476 2.16 ± 0.203 GB-151-6 Brain 0.432 <0.35 GB-134-3 Heart 0.158 1.10 ± 0.275 GB-134-3 Liver 0.523 0.91 ± 0.146 GB-134-3 Spleen 0.118 1.14 ± 0.342 GB-134-3 R&L Kidney 0.406 1.59 ± 0.191 GB-134-3 Brain 0.455 <0.25 Meso-2 Heart 0.145 1.67 ± 0.301 Meso-2 Liver 0.935 6.67 ± 0.254 Meso-2 Spleen 0.080 3.01 ± 0.572 Meso-2 R&L Kidney 0.415 7.63 ± 0.351 Meso-2 Brain 0.400 0.74 ± 0.148 Meso-2 Blood 0.268 2.05 ± 0.287 *organs from two mice were combined to make one sample