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STABILIZATION OF OXIDASES BY GLYCINE

20230048008 · 2023-02-16

    Inventors

    Cpc classification

    International classification

    Abstract

    Described are compositions and methods relating to the stabilization of oxidase enzymes using the amino acid glycine. The compositions and methods allow for drying oxidase-containing compositions with improved enzyme activity yield and long term storage of dried oxidase-containing compositions, in some cases without the need for refrigeration.

    Claims

    1. A method for increasing the stability of an oxidase enzyme in a composition, comprising; admixing with the oxidase enzyme the free amino acid glycine at a ratio of at least 1 gram glycine per gram oxidase enzyme, wherein the admixed oxidase enzyme has increased stability in the composition compared to an oxidase enzyme in an otherwise identical composition lacking glycine.

    2. The method of claim 1, wherein the ratio is at least 6.4 gram glycine per gram oxidase enzyme.

    3. The method of claim 1 or 2, wherein glycine is the primary stabilizer of oxidase enzyme in the formulation.

    4. The method of any previous claims, wherein glycine is present in the substantial absence of free acidic amino acids.

    5. The method of any previous claims, wherein glycine is the only free amino acid present.

    6. The method of any previous claims, wherein the oxidase enzyme is glucose oxidase or hexose oxidase.

    7. The method of any of the previous claims, wherein the oxidase enzyme and glycine are admixed in an aqueous solution or suspension.

    8. The method of claim 7, wherein the admixed oxidase enzyme and glycine are subsequently dried.

    9. A composition comprising an oxidase enzyme and the free amino acid glycine at a ratio of at least 1 gram glycine per gram oxidase enzyme, wherein the oxidase enzyme has increased stability in the composition compared to an oxidase enzyme in an otherwise identical composition lacking glycine.

    10. The composition of claim 9, wherein the ratio is at least 6.4 gram glycine per gram oxidase enzyme.

    11. The composition of claim 9 or 10, wherein glycine is present in the substantial absence of acidic amino acid residues.

    12. The composition of any of claims 9-11, wherein glycine is the only free amino acid present.

    13. The composition of any of claims 9-12, wherein the oxidase enzyme is glucose oxidase hexose oxidase.

    14. The method or composition of any of claims 9-13, wherein the oxidase enzyme and glycine are incorporated into a granule, a film, a pad, a gel, or other solid and/or liquid composition.

    Description

    BRIEF DESCIPTION OF THE DRAWING

    [0024] FIG. 1 is a graph showing the the ratio of bound to free FAD in the presence of increasing amounts of glycine per gram active GOx.

    DETAILED DESCRIPTION OF THE INVENTION

    I. Introduction

    [0025] The inventors have discovered that incorporation of the amino acid glycine, more than any other amino acid, improves the heat drying yield in production of enzyme compositions from formulated oxidase enzyme concentrates. While stabilization of oxidases, such as glucose oxidase (GOx), using amino acids has been described (see, e.g., U.S. Pat. No. 4,543,326), such studies have consistently identified different amino acid residues, such as acidic amino acid residues (i.e., aspartic acid and glutamic acid, and salts, thereof) as being the most preferable amino acids for stabilization. The present selection invention relates to the use of glycine, a neutral amino acid, specifically, as a preferred stabilizer of oxidases.

    II. Definitions and abbreviations

    [0026] Prior to describing the present compositions and methods in detail, the following terms are defined for clarity. Terms not defined should be accorded their ordinary meanings as used in the relevant art.

    [0027] As used herein, the term “granule” refers to a small particle of a substance. The particle comprises a core, optionally with one or more coating layers.

    [0028] As used herein, “weight percent,” “weight fraction,” “mass fraction” or simply “fraction” refers to the relative amount of mass on a % wt/wt or fractional wt/wt basis, for example, the relative amount of mass of an ingredient compared to the mass of an entire granule.

    [0029] As used herein, the terms “pellets” and “pelleting” refer to solid, rounded, spherical and cylindrical tablets or pellets and the processes for forming such solid shapes, particularly feed pellets and solid, extruded animal feed.

    [0030] As used herein, the term “recovered activity” or “activity recovery” refers to the ratio of (i) the activity of an enzyme after a treatment involving one or more of the following stressors: heating, increased pressure, increased pH, decreased pH, storage, drying, exposure to surfactant(s), exposure to solvent(s), and mechanical stress) to (ii) the activity of the enzyme before the treatment. The recovered activity may be expressed as a percentage. The percent recovered activity is calculated as follows:

    [00001] % recovered activity = ( activity after treatment ) ( activity before treatment ) × 100 %

    [0031] As used herein, the term “about” refers to ±15% to the referenced value.

    [0032] For ease of reference, elements of the present compositions and methods may be arranged under one or more headings. It is to be noted that the compositions and methods under each of the headings also apply to the compositions and methods under the other headings.

    [0033] As used herein, the singular articles “a,” “an” and “the” encompass the plural referents unless the context clearly dictates otherwise. All references cited herein are hereby incorporated by reference in their entirety. The following abbreviations/acronyms have the following meanings unless otherwise specified:

    [0034] ° C. degrees Centigrade

    [0035] g or gm gram

    [0036] g/L grams per liter

    [0037] g/mol grams per mole

    [0038] mol/mol mole to mole ratio

    [0039] μmol micromole

    [0040] hr or h hour

    [0041] kg kilogram

    [0042] mg milligram

    [0043] mL or ml milliliter

    [0044] min minute

    [0045] M molar

    [0046] mM millimolar

    [0047] μm micrometer (micron)

    [0048] μL and μl microliter

    [0049] UFC ultrafiltered concentrate

    [0050] dissolved solids active oxidase protein plus other non-oxidase fermentation solids

    [0051] RH relative humidity

    [0052] wt weight

    [0053] % wt/wt weight percent

    III. Oxidases that can be stabilized by glycine

    [0054] The discovery that glycine is the preferred amino acid stabilizer for exemplified oxidase enzymes, is expected to apply to a broad range of oxidases. Moreover, testing glycine for the ability to stabilize a particular oxidase is routine and does not require undue experimentation.

    [0055] Particular oxidases expected to be stabilized using glycine are those that use molecular oxygen (02) as an acceptor, and are classified as EC 1.1.3. Exemplary oxidases include those listed in Table 1.

    TABLE-US-00001 TABLE 1 EC 1.1.3 enzymes Enzyme classification Common name EC 1.1.3.3 malate oxidase EC 1.1.3.4 glucose oxidase EC 1.1.3.5 hexose oxidase EC 1.1.3.6 cholesterol oxidase EC 1.1.3.7 aryl-alcohol oxidase EC 1.1.3.8 L-gulonolactone oxidase EC 1.1.3.9 galactose oxidase EC 1.1.3.10 pyranose oxidase EC 1.1.3.11 L-sorbose oxidase EC 1.1.3.12 pyridoxine 4-oxidase EC 1.1.3.13 alcohol oxidase EC 1.1.3.14 catechol oxidase (dimerizing) EC 1.1.3.15 (S)-2-hydroxy-acid oxidase EC 1.1.3.16 ecdysone oxidase EC 1.1.3.17 choline oxidase EC 1.1.3.18 secondary-alcohol oxidase EC 1.1.3.19 4-hydroxymandelate oxidase EC 1.1.3.20 long-chain-alcohol oxidase EC 1.1.3.21 glycerol-3-phosphate oxidase EC 1.1.3.23 thiamine oxidase EC 1.1.3.24 L-galactonolactone oxidase EC 1.1.3.27 hydroxyphytanate oxidase EC 1.1.3.28 nucleoside oxidase EC 1.1.3.29 N-acylhexosamine oxidase EC 1.1.3.30 polyvinyl-alcohol oxidase EC 1.1.3.37 D-arabinono-1,4-lactone oxidase EC 1.1.3.38 vanillyl-alcohol oxidase EC 1.1.3.39 nucleoside oxidase (H2O2-forming) EC 1.1.3.40 D-mannitol oxidase EC 1.1.3.41 xylitol oxidase EC 1.1.3.42 prosolanapyrone-II oxidase EC 1.1.3.43 paromamine 6′-oxidase EC 1.1.3.44 6-hydroxyneomycin C oxidase

    [0056] The oxidase enzyme is preferably stabilized with glycine in an aqueous mixture but may subsequently be dried, such as by spray drying, spray agglomeration, spray granulation etc. The oxidase enzyme may be subjected to high shear and extrusion followed by drying, and may used in fluid bed coating. The glycine stabilized oxidase may be incorporated into a granule,a pellet, a film, a pad, a gel, or any other solid or liquid composition, preferably one that does not separate glycine from the oxidase.

    IV. Ratio of glycine to oxidase enzyme

    [0057] It is likely that different oxidases will require different amounts of glycine for stabilization, which amounts are readily determined. Such amounts are best expressed as the molar ratio or weight percentage of glycine to active oxidase enzyme protein or, alternatively, glycine to oxidase enzyme activity (in defined units). Based on the appended Examples, the recommended ratio is about 1 to about 10 g glycine per g active oxidase protein, for example about 1.6 to about 8.4 g glycine per g active oxidase protein. In some case, the ratio is at least about 6.4 g glycine per g active oxidase protein.

    [0058] The origin of the glycine, i.e., whether naturally occurring or synthetic, is not critical. It will be appreciated the glycine used as a stabilizer is free glycine and not glycine residues incorporated into a protein, including the oxidase protein to be stabilized. Glycine is the primary determinant for oxidase stabilization, meaning it is the only excipient necessary and sufficient for improved stability; however, glycine may also be mixed with other amino acids, other stabilizing agents, or other beneficial agents.

    EXAMPLES

    [0059] The following examples are intended to be illustratative, but not limit the scope of this invention to the exemplified oxidases. The glucose oxidase (GOx) enzyme also known as Notatin (EC number 1.1.3.4) is an oxidase that catalyzes the oxidation of glucose to hydrogen peroxide and D-glucono-δ-lactone. This enzyme is produced by certain species of fungi such as Aspergillus niger. The oxidation reaction is performed by flavin adenine dinucleotide (FAD), a redox cofactor which is tightly bound, not covalently, deep between two identical GOx monomers. The GOx dimer contains two FAD cofactors that are responsible for the oxidation-reduction properties of the enzyme. GOx is a thermally labile enzyme and is sensitive to drying processes that involve heating. Under denaturing conditions, such as those occurring during heat drying, the dimer is dissociated to its subunits, leading to irreversible loss of cofactors, transitioning from the “bound” to “free” state, which in turn leads to enzyme inactivation and aggregation.

    Example 1. Thermal inactivation of GOx during heat drying

    [0060] Two samples of neat (unformulated) GOx UFC (25 mg active protein per g UFC) were obtained from DuPont/Danisco fermentation plants. The samples were incubated in an oven at 50° C. for four, eight and twenty-four hours. The experimental method involved addition of 80 μL of each sample to interior wells of a 96-well plate (to avoid edge effects), sealing the plate with breathable seal, and incubaring the plate at 50° C. The weight of the plate was recorded before and after drying to ensure all water was removed.

    [0061] To measure activity, the dried content of each well was re-suspended in 80 μL of purified water. After resuspension, the activity was measured using a standard glucose oxidase assay. Glucose oxidase catalyzes the conversion of glucose and oxygen to hydrogen peroxide and gluconic acid in the assay. A reaction of hydrogen peroxide with 2,2′-azino-bis(3-ethylbenzthiazolin-6-sulfonsyre), ABTS, changes the appearance of reaction media from colorless to green. This reaction is catalyzed by the enzyme peroxidase. The green color is measured on a spectrophotometer at 405 nm. The method is calibrated using a linear regression of standard dilutions prepared from a standard material with a known concentration. The oxidase enzymatic activity decreased with time as shown in Table 2.

    TABLE-US-00002 TABLE 2 The oxidase activity yields of neat GOx UFC samples incubated at 50° C. for 4, 8, and 24 hours; n = 8, avg. ± stdev % Recovered Activity Unformulated GOx UFC 4 hr 8 hr 24 hr Sample #1 81% ± 2.8% 52% ± 3.4%  31% ± 3.6% Sample #2 71% ± 4.8% 34% ± 7.4% 13% ± 11%

    Example 2. Thermal stabilization of GOx by glycine

    [0062] A sample of neat (unformulated) GOx UFC (25 mg active protein per g UFC) was obtained from a DuPont/Danisco fermentation plant. A series of thermal stress experiments was conducted on the GOx concentrate formulated with different concentrations of glycine ranging from 0%-16%. A correlation was observed between GOx denaturation (based on the ratio of the bound to free FAD cofactors) and glycine concentration after heating the samples for 8 hours at 50° C. (Table 3). FAD profiling of GOx samples was performed by hydrophobic interaction chromatography with UV detection at 450 nm. The area under the absorption curve vs. retention time was determined for “bound” and “free” FAD cofactors, and their respective ratio was then calculated. Addition of glycine to the GOx UFC reduced the degree of denaturation of enzyme protein under the heat stress. Based on graphical analysis of the denaturation profile, preferred glycine concentrations are greater than about 1 g glycine per g oxidase protein, for example greater than 1.6, or even greater than 6.4 g glycine per g oxidase protein. Amounts greater than about 8.4 g glycine per g oxidase protein do not apper to provide much additional benefit.

    TABLE-US-00003 TABLE 3 Variation of free and bound FAD with glycine concetration % Glycine to Glycine to Gox Conc. Gox Mass Ratio Bound Ratio (g glycine/ to Free (w glycine/ g active Free Bound FAD w UFC) protein) FAD FAD Ratio 0% 0 184.7 545.9 3.0 4% 1.6 126.7 805.7 6.4 8% 3.2 83.2 761.5 9.2 16%  6.4 61.3 784.4 12.8

    [0063] Samples of neat GOx UFC and formulated GOx UFC containing a cationic or neutral amino acid were prepared for drying in a 96-well plate. About 20 μL of each GOx preparation was added to 6 wells and the plate was sealed with a breathable cover. The plate was incubated at 50° C. for 4 hours to dry the samples. Enzyme activity of dried samples was measured by the protocol descrbed in Example 1 above.

    [0064] Cationic amino acids included arginine and lysine, and neutral amino acids included alanine, glycine, proline, and threonine. Among the amino acids tested, alanine, glycine and proline showed the highest solubility in the GOx UFC. Histidine, a neutral amino acid, was not included, despite its high solubility, due to its tendency to increase the pH of the concentrate.

    [0065] The recovered activity of GOx formulated with different cationic and neutral amino acids is shown in Table 4. Anionic amino acids including aspartic acid, D-glutamic acid, and L-glutamic acid had considerably lower solubility in the GOx UFC, and showed inferior enzyme activity yield compared to neutral and cationic amino acids. As such, they are not preferred excipients for thermal stabilization of GOx compositions of this invention.

    TABLE-US-00004 TABLE 4 Recovered activity of GOx after drying at 50° C. for 4 hours; n = 6, avg ± stdev AA to GOx AA to GOx AA side mass ratio mass ratio Amino chain (g AA/ (mM AA/ Recovered acid charge at g active g active activity (AA) pH 7.4 protein) protein) (%) — — 0 0 73.87% ± 5.43% Arginine positive 3.8 21.81 73.73% ± 6.63% Lysine positive 3.7 25.31 93.63% ± 7.70% Alanine neutral 4.0 44.90 88.74% ± 6.46% Glycine neutral 4.0 53.29 102.38% ± 6.80%  Proline neutral 4.1 35.61 88.44% ± 8.76% Theronine neutral 3.9 32.74 91.35% ± 8.59%

    [0066] The activity assay results showed that the dried formulation with glycine had the highest recovered activity compared to the neat sample without glycine and the samples formulated with other neutral and cationic amino acids. Glycine has the lowest molecular weight among other amino acids tested, enabling its incorporation as a thermal stabilizer at the highest molar concentration relative to active enzyme protein.

    Example 3. Storage stability of GOx spray dried compositions

    [0067] Addition of glycine to GOx concentrate, UFC dissolved solids 8.2%, at 14% (wt glycine/wt UFC), i.e. 5.6 g glycine per g active protein, improved the storage stability of dried enzyme composition produced with spray drying. The spray dried GOx powder compositions with glycine and without glycine (control) were subjected to a 6-month stability study. The samples were contained in closed cap plastic bottles and incubated at 37° C. and 65% relative humidity for 180 days. The enzyme activity was monitored during this period by analyzing the samples after 0, 3, 7, 14, 30, 60, 90 and 180 days. The recovered enzymatic activity of the tested samples is tabulated in Table 5. The GOx/glycine composition maintained up to 55% of enzyme activity after 180 days in storage.

    TABLE-US-00005 TABLE 5 Recovered enzymatic activity (%) of glucose oxidase/glycine spray dried powder composition in comparison with the unformulated glucose oxidase after 6-month storage at 37° C./65% RH Time (days) 0 3 7 14 30 60 90 180 Samples Recovered activity (%) Unformulated 100 86 86 75 74 61 50 28 GOx/glycine 100 90 88 80 81 69 60 55