Solid fibrinogen preparation
09775884 · 2017-10-03
Assignee
Inventors
- Shinichi Miyagawa (Kumamoto, JP)
- Tatsuya Araki (Kumamoto, JP)
- Tsutomu Hamuro (Kumamoto, JP)
- Mika Okuda (Kumamoto, JP)
- Hiroshi Kaetsu (Kumamoto, JP)
Cpc classification
A61K31/198
HUMAN NECESSITIES
A61P7/04
HUMAN NECESSITIES
A61K31/198
HUMAN NECESSITIES
A61K2300/00
HUMAN NECESSITIES
A61K2300/00
HUMAN NECESSITIES
C12Y203/02013
CHEMISTRY; METALLURGY
International classification
A61K31/198
HUMAN NECESSITIES
Abstract
A fibrinogen preparation is provided which has an improved solubility, may be prepared within a short time and may be used rapidly in clinical set-up. A solid fibrinogen preparation comprising as a main ingredient fibrinogen and further containing the following components: albumin; a nonionic surfactant; a basic amino acid or a salt thereof; and at least two amino acids or a salt thereof selected from an acidic amino acid or a salt thereof and a neutral amino acid or a salt thereof. The solid fibrinogen composition of the present invention may be held on a medical material to form a supporting material holding fibrinogen. Besides, the supporting material holding fibrinogen may be combined with a component comprising as a main ingredient thrombin to provide a fibrin adhesive.
Claims
1. A solid fibrinogen composition comprising fibrinogen, albumin, a non-ionic surfactant and a combination of amino acid or amino acid salts selected from the group consisting of: isoleucine, glycine, arginine, and glutamic acid, or salts thereof (IGRE); glycine, arginine, and glutamic acid, or salts thereof (GRE); isoleucine, glycine, and arginine, or salts thereof (IGR); leucine, glycine, arginine, and glutamic acid, or salts thereof (LGRE); isoleucine, alanine, arginine, and glutamic acid, or salts thereof (IARE); isoleucine, serine, arginine, and glutamic acid, or salts thereof (ISRE); isoleucine, threonine, arginine, and glutamic acid, or salts thereof (ITRE); isoleucine, glutamine, arginine, and glutamic acid, or salts thereof (IQRE); and isoleucine, glycine, lysine and glutamic acid, or salts thereof (IGKE).
2. The solid fibrinogen composition of claim 1, wherein the surfactant is tyloxapol or polysorbate 80.
3. The solid fibrinogen composition of claim 1, further comprising at least one of a monofilament, cotton, paper, cellulose, cellulose derivative, nonwoven fabric, textile, knit, sponge, film or other supporting material.
4. The solid composition of claim 1, further comprising at least one of collagen, gelatin, polyglycolic acid, polylactic acid, glycolic acid-lactic acid copolymer, polyglutamic acid, or amylose.
5. The solid fibrinogen composition of claim 1 in a lyophilized form and suitable for medical use.
6. A liquid composition produced by contacting water with the solid fibrinogen composition of claim 1.
7. The liquid composition of claim 6 that rehydrates faster or that has a shorter defoaming time than an otherwise identical composition produced by contacting water with a solid fibrinogen composition that does not contain at least one of albumin, a non-ionic surfactant, or one of the amino acids or amino acid salts in the combination of amino acids or amino acid salts.
8. A solid fibrinogen composition comprising fibrinogen, albumin, a non-ionic surfactant, and a combination of amino acids or amino acid salts selected from the group consisting of: glycine or a glycine salt, arginine or a salt of arginine, glutamic acid or a salt of glutamic acid (GRE); and isoleucine or an isoleucine salt, glycine or a glycine salt, arginine or a salt of arginine, (IGR).
9. The solid fibrinogen composition of claim 8, wherein the surfactant is tyloxapol or polysorbate 80.
10. The solid fibrinogen composition of claim 8, further comprising at least one of a monofilament, cotton, paper, cellulose, cellulose derivative, nonwoven fabric, textile, knit, sponge, film or other supporting material.
11. The solid fibrinogen composition of claim 8, further comprising at least one of collagen, gelatin, polyglycolic acid, polylactic acid, glycolic acid-lactic acid copolymer, polyglutamic acid, or amylose.
12. The solid fibrinogen composition of claim 8 in a lyophilized form and suitable for medical use.
13. A liquid composition produced by contacting water with the solid fibrinogen composition of claim 8.
14. The liquid composition of claim 13 that rehydrates faster or that has a shorter defoaming time than an otherwise identical composition produced by contacting water with a solid fibrinogen composition that does not contain at least one of albumin, a non-ionic surfactant, or one of the amino acids or amino acid salts in the combination of amino acids or amino acid salts.
15. A solid fibrinogen composition comprising fibrinogen, albumin, a non-ionic surfactant, and isoleucine or an isoleucine salt, glycine or a glycine salt, arginine or a salt of arginine, glutamic acid or a salt of glutamic acid (IGRE).
16. The solid fibrinogen composition of claim 15, wherein the surfactant is tyloxapol or polysorbate 80.
17. The solid fibrinogen composition of claim 15, further comprising at least one of a monofilament, cotton, paper, cellulose, cellulose derivative, nonwoven fabric, textile, knit, sponge, film or other supporting material.
18. The solid fibrinogen composition of claim 15, further comprising at least one of collagen, gelatin, polyglycolic acid, polylactic acid, glycolic acid-lactic acid copolymer, polyglutamic acid, or amylose.
19. A liquid composition produced by contacting water with the solid fibrinogen composition of claim 15.
20. The liquid composition of claim 19 that rehydrates faster or that has a shorter defoaming time than an otherwise identical composition produced by contacting water with a solid fibrinogen composition that does not contain at least one of albumin, a non-ionic surfactant, isoleucine or an isoleucine salt, glycine or a glycine salt, arginine or a salt of arginine, or glutamic acid or a salt of glutamic acid.
Description
BRIEF DESCRIPTION OF DRAWINGS
(1)
(2)
(3)
(4)
BEST MODE FOR CARRYING OUT THE INVENTION
(5) The solid fibrinogen preparation of the present invention comprises fibrinogen as a main ingredient and a substantially necessary amount of albumin, a nonionic surfactant, a basic amino acid, and two or more amino acids selected from an acidic amino acid or a neutral amino acid in a suitable buffer solution such as a solution containing sodium chloride, trisodium citrate.
(6) A concentration of fibrinogen comprised in the preparation of the present invention is preferably 40 mg/mL or more, more preferably 80 mg/mL or more.
(7) Albumin contained in the preparation of the present invention is preferably serum albumin. Human serum albumin is preferred when the preparation of the present invention is applied to human. A concentration of albumin comprised in the preparation of the present invention is preferably 5 mg/mL or more. The upper limit of the concentration may suitably be decided based on the common knowledge in the art and include but not limited to 15 mg/mL.
(8) A nonionic surfactant comprised in the preparation of the present invention includes a fatty acid surfactant such as sucrose fatty acid ester, sorbitan fatty acid ester, polyoxyethylene sorbitan fatty acid ester, fatty acid alkanolamide and the like, a higher alcohol surfactant such as polyoxyethylene alkyl ether, alkyl glycoside and the like, and an alkylphenol surfactant such as polyoxyethylene alkyl phenyl ether and the like. Among these, a suitable example is Tween-surfactant and Triton-surfactant. An example of these suitable nonionic surfactants includes polyoxyethylene(20) sorbitan monooleate (Tween80) and tyloxapol.
(9) A concentration of said nonionic surfactant need to be over the critical micellar concentration of each surfactant and preferably is 0.1 mg/mL or more. The upper limit of the concentration may suitably be decided based on the common knowledge in the art and include but not limited to 0.5 mg/mL.
(10) The basic amino acid comprised in the preparation of the present invention is selected from any of arginine or a salt thereof and lysine or a salt thereof.
(11) For the acidic amino acid or the neutral amino acid comprised in the preparation of the present invention, two or more amino acids may be selected from an acidic amino acid such as glutamic acid, aspartic acid, or a salt thereof, or a neutral amino acid such as isoleucine, leucine, glycine, alanine, serine, threonine, glutamine, or a salt thereof.
(12) In addition, for the said acidic amino acid or the neutral amino acid, at least two amino acids or a salt thereof may be selected from at least 2 of the following groups: (1) glutamic acid, or aspartic acid; (2) isoleucine, or leucine; (3) glycine, alanine, serine, threonine, or glutamine.
(13) Moreover, a preferred combination of said basic amino acid with said acidic amino acid or neutral amino acid includes the following: arginine, glutamic acid and isoleucine, or a salt thereof; arginine, glutamic acid and glycine, or a salt thereof; arginine, glycine and isoleucine, or a salt thereof; arginine, isoleucine, glycine and glutamic acid, or a salt thereof; lysine, isoleucine, glycine and glutamic acid, or a salt thereof; arginine, leucine, glycine and glutamic acid, or a salt thereof; arginine, isoleucine, alanine and glutamic acid, or a salt thereof; arginine, isoleucine, serine and glutamic acid, or a salt thereof; arginine, isoleucine, threonine and glutamic acid, or a salt thereof; arginine, isoleucine, glutamine and glutamic acid, or a salt thereof; arginine, isoleucine, glycine and aspartic acid, or a salt thereof.
(14) A concentration of each amino acid or a salt thereof comprised in the preparation of the present invention is preferably 2 mg/mL or more. In case of a particularly preferred combination of the amino acids, including arginine, isoleucine, glycine and glutamic acid, a concentration of each amino acids is preferably 3 mg/mL or more, 3 mg/mL or more, 2 mg/mL or more and 2.5 mg/mL or more, respectively. The upper limit of the concentration may suitably be decided based on the common knowledge in the art and include but not limited to 36 mg/mL, 13 mg/mL, 15 mg/mL, and 30 mg/mL, respectively.
(15) Factor XIII may be added additionally to the fibrinogen preparation of the present invention in order to enhance the physical strength and stability of the fibrin clot. A concentration of Factor XIII comprised in the preparation of the present invention is such that the cross-link of isopeptide linkage between fibrin molecules, i.e. γ dimer, may be formed and is preferably e.g. 0.4 unit or more/mL of the preparation.
(16) A method for preparing fibrinogen, albumin and Factor XIII used in the present invention is not particularly limited and includes e.g. separation from human blood or by genetic recombination technique.
(17) Fibrinogen, a main ingredient of the preparation of the present invention, may be prepared by known methods, including, for example, cold ethanol precipitation combined with glycine that decreases solubility of fibrinogen (Blomback, B. and Blomback, M., Arkiv Kemi, 10, p. 415-443 (1956)), and glycine precipitation using glycine alone (Kazal, L. A. et al., Proc. Soc. Exp. Biol. Med., 113, p. 989-994 (1963)), and the like as reported. Alternatively, fibrinogen produced by genetic recombination technique may also be used.
(18) Factor XIII may be prepared by known methods, including, for example, purification from plasma (Curtis, C G., Lorand, L., Methods Enzymol., 45, p. 177-191 (1976)) as reported. Alternatively, Factor XIII produced by genetic recombination technique may also be used.
(19) The fibrinogen preparation of the present invention, in addition to being provided in a dosage form contained in a vial, may be held on a medical material to form a supporting material holding fibrinogen.
(20) Specifically, a medical material may be soaked in the fibrinogen solution comprised of the composition of the present invention and then dried, e.g. by lyophilization, to produce a supporting material holding fibrinogen.
(21) An example of said supporting material is not particularly limited insofar as it may medically be used and includes for example cellulose, a cellulose derivative, collagen, gelatin, polyglycolic acid, polylactic acid, glycolic acid-lactic acid copolymer, polyglutamic acid, amylose, and the like. The supporting material may be in the form including a fiber assembly such as monofilament, cotton, paper, nonwoven fabric, textile, and knit, film, sponge, and the like. A preferable example is a nonwoven fabric of polyglycolic acid, bioabsorbable material, as used in Examples in the specification.
(22) Besides, the fibrinogen preparation and the supporting material holding fibrinogen of the present invention may not only be used alone but also in combination with a component comprising thrombin as a main ingredient to thereby form a biological adhesive (fibrin adhesive) for human and animal tissue that may broadly be applicable in the clinical set-up.
(23) The present invention is explained in more detail by means of the following Test and Examples but is not limited thereto.
EXAMPLE
(24) Test: Test and Method
(25) (1) Preparation of the Fibrinogen Lyophilized Powder
(26) Domestic frozen donation-plasma were thawed at low temperature and the resulting cryoprecipitate were treated by a combination of cold ethanol precipitation and glycine precipitation to produce fibrinogen. A fibrinogen solution for use in lyophilization was prepared by dissolving fibrinogen in a citric acid buffer solution containing sodium chloride and then adding each additives (prepared at ¼ of the final concentration). The resulting fibrinogen solution was subjected to aseptic filtration and each 12 mL was dispensed into final containers (glass bottles), which were then lyophilized and hermetically sealed.
(27) (2) Rehydration Time
(28) Rehydration time was determined as a time necessary for complete dissolution at 23 to 26° C. after 3 mL of the solvent (H.sub.2O) was added to the lyophilized powder. For dissolving the lyophilized powder, the vial container containing the solvent was vigorously shook by hand. A content of a coagulable protein (fibrinogen) upon dissolution was set to 80 mg/mL to 90 mg/mL. Rehydration time was reported as a mean (±SD) of four measurements.
(29) (3) Defoaming Time
(30) Defoaming time was determined as a total time from the point when the lyophilized powder was dissolved and left to stand at room temperature until the bubble formed on dissolution disappeared and the surface of the fibrinogen solution appeared. Defoaming time was reported as a mean (±SD) of three measurements.
(31) (4) Content of Coagulable Protein (Fibrinogen)
(32) A content of coagulable protein (fibrinogen) was determined according to the tests for clottable protein content and purity, which is a test for itemized product and is described in Notification of the Welfare Ministry, “MINIMUM REQUIREMENTS FOR BIOLOGICAL PRODUCTS”. Briefly, an amount of proteins precipitated upon addition of thrombin to samples is determined. Purity of the material used in Examples (a ratio of the amount of coagulable protein to total proteins) was 90% or more. A content of fibrinogen described in Examples was reported as a mean of two measurements.
(33) (5) Preparation of a Fibrinogen Sheet
(34) A fibrinogen sheet was prepared by soaking a sheet of polyglycolic acid (Gunze: Neoveil (registered trademark)), a sheet-shaped medical material, with a fibrinogen solution at 50 μL/cm.sup.2, followed by lyophilization. A fibrinogen sheet was prepared such that it has a final concentration of fibrinogen of 80 mg/mL to 90 mg/mL when the fibrinogen sheet is rehydrated with 50 μL/cm.sup.2 of saline.
(35) (6) Saturation Time of the Fibrinogen Sheet with Saline
(36) A saturation time was determined as a time (second) from dropwise addition of saline (200 μL) onto fibrinogen sheet (2×2 cm) to completion of absorption of saline into the sheet while left standing. A saturation time was reported as a mean (±SD) of three measurements.
(37) (7) Tensile Strength Test
(38) A tensile strength of the fibrinogen sheet was determined by the method described in ASTM (American Society for Testing and Materials) (F2258: Standard Test) with some modification. First, 2 sheets of pig dermis were obtained and fixed by fixtures separately (2.5×2.5 cm). Next, 300 μL of 30 U/mL thrombin was absorbed into the pig dermis sheets and a fibrinogen sheet (2.5×2.5 cm) was tucked between these dermis and left to stand for 1 to 5 min. After that, a tensile strength was determined while the pig dermis sheets were pulled upward and downward at 2 mm/min of a moving rate. A content of a coagulable protein (fibrinogen) upon dissolution was set to 80 mg/mL to 90 mg/mL.
(39) (8) Other Reagents
(40) As used in the following Examples, NaCl was purchased from Tomita pharmaceutical Co., Ltd. Trisodium citrate dihydrate, serine, threonine, glutamine, leucine, alanine and isoleucine were purchased from Wako Pure Chemical Industries, Ltd. Glycine, arginine monohydrochloride, sodium glutamate, sodium aspartate, lysine monohydrochloride and tyloxapol (Triton WR-1339) were purchased from nacalai tesque and Tween80 was purchased from NOF CORPORATION. Albumin was purified from domestic plasma donations at Juridical Foundation the Chemo-Sero-Therapeutic Research Institute.
Example 1: Rehydration Time Relative to Prior Art
(41) A lyophilized fibrinogen powder was prepared comprising fibrinogen as a main ingredient, a substantively necessary amount of albumin, isoleucine or glycine for a neutral amino acid, arginine monohydrochloride for a basic amino acid, sodium glutamate for an acidic amino acid, and Tween80 or tyloxapol for a surfactant, and rehydration time was determined upon addition of the solvent.
(42) A lyophilized fibrinogen powder composition of the present invention was prepared comprising, upon rehydration, 84 mg/mL or more of fibrinogen, 17.5 mg/mL of NaCl, 12 mg/mL of trisodium citrate dihydrate, 10 mg/mL of HSA (human serum albumin), 0.2 mg/mL of Tween80 or 0.3 mg/mL of tyloxapol, isoleucine, glycine, arginine monohydrochloride and sodium glutamate and a rehydration time was determined as described above. Besides, as a prior art, lyophilized powders were prepared by reference to fibrinogen compositions described in the instructions of commercially available fibrin glue adhesives (three kinds) and a rehydration time was determined in the same way for comparison with those of the composition of the present invention.
(43) Table 1 shows compositions, concentrations of each component, and a content of coagulable protein (fibrinogen) upon dissolution. In addition,
(44) TABLE-US-00001 TABLE 1 Composition Composition No Additive No. 1 No. 2 No. 3 Prior art 1 Prior art 2 Prior art 3 NaCl(mg/mL) 17.5 17.5 17.5 17.5 15 3 Trisodium citrate (mg/mL) 12 12 12 12 5 6 Albumin (mg/mL): Al 10 10 10 10 15 15 Isoleucine (mg/mL): I 4 4 13 — 13 — Glycine (mg/mL): G 3 3 3 15 — 25 Arginine 12 12 36 — 12 — monohydrochloride(mg/mL): R Sodium glutamate (mg/mL): E 10 10 10 — 10 — Mannitol (mg/mL) — — — 40 — — Aprotinin (unit/mL) — — — — — 60 Tween80(mg/mL): De 0.2 — 0.2 — — Tyloxapol (mg/mL): De — 0.3 — — — 0.3 Content of Coagulable 86 88 86 85 85 84 Protein (mg/mL)
Example 2: Additives Required to Reduce Rehydration Time
(45) There were prepared a lyophilized fibrinogen powder composition comprising, upon rehydration, 4 mg/mL of isoleucine (I), 2 mg/mL of glycine (G), 12 mg/mL of arginine monohydrochloride (R), 10 mg/mL of sodium glutamate (E), 10 mg/mL of HSA (human serum albumin: Al) and 0.2 mg/mL of Tween80(De) in addition to 84 mg/mL or more of fibrinogen, 17.5 mg/mL of NaCl and 12 mg/mL of trisodium citrate dihydrate (IGRE-AlDe) as well as lyophilized fibrinogen powder compositions comprising the composition of IGRE-AlDe with removal of any one of HSA, isoleucine, glycine, arginine monohydrochloride, sodium glutamate, or Tween80 (IGRE-De, GRE-AlDe, IRE-AlDe, IGE-AlDe, IGR-AlDe, and IGRE-Al, respectively). A rehydration time was determined as described above. Besides, as a prior art, the lyophilized fibrinogen powders of the compositions of Prior art 1 to Prior art 3 as used in Example 1 were prepared and a rehydration time was determined for comparison with those of the compositions as described above.
(46) Table 2 shows compositions, concentrations of each component, and a content of coagulable protein (fibrinogen) upon dissolution. In addition,
(47) TABLE-US-00002 TABLE 2 Composition Composition IGRE- IGRE-De GRE-AlDe IRE-AlDe IGE-AlDe IGR-AlDe IGRE-Al Prior Prior Prior Additive AlDe (Δ HSA) (Δ Ile) (Δ Gly) (Δ Arg) (Δ Glu) (Δ detergent) art1 art2 art3 NaCl(mg/mL) 17.5 17.5 17.5 17.5 17.5 17.5 17.5 17.5 15 3 Trisodium citrate(mg/mL) 12 12 12 12 12 12 12 12 5 6 Albumin(mg/mL): Al 10 — 10 10 10 10 10 10 15 15 Isoleucine(mg/mL): I 4 4 — 4 4 4 4 — 13 — Glycine(mg/mL): G 3 3 3 — 3 3 3 15 — 25 Arginine 12 12 12 12 — 12 12 — 12 — monohydrochloride(mg/mL): R Sodium glutamate(mg/mL): E 10 10 10 10 10 — 10 — 10 — Mannitol(mg/mL) — — — — — — — 40 — — Aprotinin(unit/mL) — — — — — — — — — 60 Tween80(mg/mL): De 0.2 0.2 0.2 0.2 0.2 0.2 — — — Tyloxapol(mg/mL): De — — — — — — — — — 0.3 Content of Coagulable 86 87 88 88 88 86 87 86 85 84 Protein(mg/mL)
Example 3: Rehydration Time on Replacement of Amino Acids
(48) There were prepared a lyophilized fibrinogen powder composition comprising the composition, upon rehydration, of IGRE-AlDe as prepared in Example 2 as well as lyophilized fibrinogen powder compositions comprising the composition of IGRE-AlDe with replacement of each one of the four amino acids with other amino acids. A rehydration time was determined as described above. Besides, as a prior art, the lyophilized fibrinogen powder of the composition of Prior art 2 as used in Example 1 was prepared and a rehydration time was determined for comparison with those of the compositions of the present invention.
(49) Compositions Comprising IGRE-AlDe with Replacement of Amino Acids
(50) Replacement of Isoleucine (I):
(51) Isoleucine (I) was replaced with leucine (L), a neutral amino acid (LGRE-AlDe).
(52) Replacement of Glycine (G):
(53) Glycine (G) was replaced with alanine (A), serine (S), threonine (T) or glutamine (Q), neutral amino acids (IARE-AlDe, ISRE-AlDe, ITRE-AlDe, IQRE-AlDe, respectively).
(54) Replacement of Arginine (R):
(55) Arginine (R) was replaced with lysine (K), classified as a basic amino acid likewise arginine (IGKE-AlDe).
(56) Replacement of Glutamic Acid (E):
(57) Glutamic acid (E) was replaced with aspartic acid (D), classified as an acidic amino acid likewise glutamic acid (IGRD-AlDe).
(58) Table 3 shows compositions, concentrations of each component, and a content of coagulable protein (fibrinogen) upon dissolution. In addition,
(59) TABLE-US-00003 TABLE 3 Composition Composition IGRE- LGRE-AlDe IARE-AlDe ISRE-AlDe ITRE-AlDe IQRE-AlDe IGKE-AlDe IGRD-AlDe Prior Additive AlDe (Ile.fwdarw.Leu) (Gly.fwdarw.Ala) (Gly.fwdarw.Ser) (Gly.fwdarw.Thr) (Gly.fwdarw.Gln) (Arg.fwdarw.Lys) (Glu.fwdarw.Asp) art NaCl(mg/mL) 17.5 17.5 17.6 17.5 17.5 17.5 17.5 17.5 15 Trisodium citrate(mg/mL) 12 12 12 12 12 12 12 12 5 Albumin(mg/mL): Al 10 10 10 10 10 10 10 10 15 Isoleucine(mg/mL): I 4 — 4 4 4 4 4 4 13 Glycine(mg/mL): G 3 3 — — — — 3 3 — Arginine 12 12 12 12 12 12 — 12 12 monohydrochloride(mg/mL): R Sodium glutamate(mg/mL): E 10 10 10 10 10 10 10 — 10 Leucine(mg/mL): L — 4 — — — — — — — Alanine(unit/mL): A — — 3 — — — — — — Serine(unit/mL): S — — — 3 — — — — — Threonine(unit/mL): T — — — — 3 — — — — Glutamine(unit/mL): Q — — — — — 3 — — — Lysine monohydrochloride — — — — — — 12 — — (unit/mL): K Sodium aspartate(unit/mL): D — — — — — — — 10 — Tween80(mg/mL): De 0.2 0.2 0.2 0.2 0.2 0.2 0.2 0.2 — Content of Coagulable 86 88 88 88 87 87 86 87 85 Protein(mg/mL)
(60) TABLE-US-00004 TABLE 4 Neutral amino acid Basic amino acid Acidic amino acid Isoleucine Glycine Arginine Glutamic acid Replaceable Leucine Alanin Lysine Aspartic Serine acid Threonine Glutamine
Example 4: Defoaming Effect with Surfactant
(61) There were prepared a lyophilized fibrinogen powder composition comprising the composition, upon rehydration, of IGRE-AlDe as prepared in Example 2 as well as lyophilized fibrinogen powder compositions comprising the composition of IGRE-AlDe with removal of either Tween80 or one of the amino acids. A defoaming time upon rehydration was determined.
(62) Table 5 shows compositions, concentrations of each component, a content of coagulable protein (fibrinogen) upon dissolution and a defoaming time. As a result, the defoaming could be detected around 2.5 to 6 min. for the compositions containing a surfactant: IGRE-AlDe, IGRE-AlDe (with replacement of Tween80 with tyloxapol), GRE-AlDe, IRE-AlDe and IGR-AlDe whereas the composition not containing surfactant IGRE-Al required 121 min. for defoamation. This demonstrated that the addition of a surfactant allowed for prompt extinction of foams resulting from rehydration of the lyophilized fibrinogen powder.
(63) TABLE-US-00005 TABLE 5 Composition Composition IGRE-AlDe IGRE- (Tween80.fwdarw. IGRE-Al GRE-AlDe IRE-AlDe IGR-AlDe Additive AlDe tyloxapol) (Δ Tween80) (Δ Ile) (Δ Gly) (Δ Glu) NaCl(mg/mL) 17.5 17.5 17.5 17.5 17.5 17.5 Trisodium citrate (mg/mL) 12 12 12 12 12 12 Albumin(mg/mL): Al 10 10 10 10 10 10 Isoleucine(mg/mL): I 4 4 4 — 4 4 Glycine(mg/mL): G 3 3 3 3 — 3 Arginine 12 12 12 12 12 12 monohydrochloride(mg/mL): R Sodium glutamate(mg/mL): E 10 10 10 10 10 — Mannitol(mg/mL) — — — — — — Aprotinin(unit/mL) — — — — — — Tween80(mg/mL): De 0.2 — — 0.2 0.2 0.2 Tyloxapol(mg/mL): De — 0.3 — — — — Content of Coagulable 86 86 84 88 88 86 Protein (mg/mL) Defoaming time (Mean ± SD min) 5.3 ± 2.5 min 2.3 ± 0.6 min 121.0 ± 14.7 min 4.0 ± 2.0 min 6.0 ± 1.0 min 4.7 ± 0.6 min
Example 5: Saturation Property and Tensile Strength of Fibrinogen Sheet
(64) The fibrinogen solutions of the composition of IGRE-AlDe prepared in Example 2, of the composition of IGRE-AlDe with removal of isoleucine or glutamic acid (GRE-AlDe, IGR-AlDe, respectively) and of the composition of a commercially available fibrin glue adhesive (Prior art to 3) were used to prepare fibrinogen sheets and a saturation time and a tensile strength were determined.
(65) Table 6 shows compositions, concentrations of each component upon addition of saline and a saturation time. In addition,
(66) These results prove that, in fact, a potent adhesion could be obtained without the procedure of dissolution of a lyophilized powder in a solution, which has commonly been used in the prior art. Thus, it is expected that the use of the solid fibrinogen preparation comprising the composition of the present invention allows for provision of a preparation capable of exerting a potent adhesion in a short time.
(67) TABLE-US-00006 TABLE 6 Composition Composition IGRE- GRE-AlDe IGR-AlDe Prior Prior Prior Additive AlDe (Δ Ile) (Δ Glu) art 1 art 2 art 3 NaCl(mg/mL) 17.5 17.5 17.5 18 15 3 Trisodium citrate(mg/mL) 12 12 12 12 5 6 Albumin(mg/mL): Al 10 10 10 10 15 15 Isoleucine(mg/mL): I 4 — 4 — 13 — Glycine(mg/mL): G 3 3 3 15 — 25 Arginine 12 12 12 — 12 — monohydrochloride(mg/mL): R Sodium glutamate(mg/mL): E 10 10 — — 10 — Mannitol(mg/mL) — — — 40 — — Aprotinin(unit/mL) — — — — — 60 Tween80(mg/mL): De 0.2 0.2 0.2 — — — Tyloxapol(mt/mL): De — — — — — 0.3 Saturation time 6.5 ± 1.0 sec 8.9 ± 4.1 sec 9.0 ± 0.9 sec 600 sec 600 sec 600 sec (Mean ± SD sec) or more or more or more
INDUSTRIAL APPLICABILITY
(68) In accordance with the present invention, a solid fibrinogen preparation may be provided that is rehydrated to a liquid state in a shorter time than the preparations using the prior art. The fibrinogen preparation of the present invention, due to its reduced rehydration time, has an advantage that it may be used more quickly at emergency. Additionally, the fibrinogen preparation of the present invention has another advantage that, due to a defoaming effect of a surfactant, a reconstituted fibrinogen solution may be quickly sucked into an applicator to thereby further reduce the preparation time.
(69) Moreover, the fibrinogen composition obtained by the present invention may preliminarily be held on a supporting material to provide a fibrinogen preparation which is directly applicable to an affected area without rehydration with a solution. The fibrinogen preparation of the present invention which is held on the supporting material may dissolve quickly with a slight amount of water on the applied area to thereby exert a strong adhesive force in a shorter time.