CN106337044A - Thrombin solution - Google Patents

Thrombin solution Download PDF

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CN106337044A
CN106337044A CN201610874955.9A CN201610874955A CN106337044A CN 106337044 A CN106337044 A CN 106337044A CN 201610874955 A CN201610874955 A CN 201610874955A CN 106337044 A CN106337044 A CN 106337044A
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thrombin
thrombin solution
acid
water
sodium
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CN106337044B (en
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余海跃
陈其云
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Sichuan Maker Biological Science And Technology Co Ltd
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Sichuan Maker Biological Science And Technology Co Ltd
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    • C12N9/00Enzymes; Proenzymes; Compositions thereof; Processes for preparing, activating, inhibiting, separating or purifying enzymes
    • C12N9/96Stabilising an enzyme by forming an adduct or a composition; Forming enzyme conjugates
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    • C12N9/48Hydrolases (3) acting on peptide bonds (3.4)
    • C12N9/50Proteinases, e.g. Endopeptidases (3.4.21-3.4.25)
    • C12N9/64Proteinases, e.g. Endopeptidases (3.4.21-3.4.25) derived from animal tissue
    • C12N9/6421Proteinases, e.g. Endopeptidases (3.4.21-3.4.25) derived from animal tissue from mammals
    • C12N9/6424Serine endopeptidases (3.4.21)
    • C12N9/6429Thrombin (3.4.21.5)
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    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/56Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving blood clotting factors, e.g. involving thrombin, thromboplastin, fibrinogen
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    • C12Y304/21005Thrombin (3.4.21.5)
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    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/86Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving blood coagulating time or factors, or their receptors

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Abstract

The invention discloses a stabilizer of a thrombin solution, the thrombin solution, a relevant detection reagent, a method for preparing a stable thrombin solution and application of the stabilizer of the thrombin solution.

Description

Thrombin solution
Technical field
The present invention relates to enzyme industrial circle and field of immunodetection, relate in particular to thrombin solution stabilizer, The detectable of thrombin solution and correlation, prepare the method for stable thrombin solution and the stabilizer of thrombin solution Purposes.
Background technology
Fibrinogen (fibrinogen, fib) is the fibrinous precursor of the main protein as blood clot Matter, is produced by hepatic parenchymal cellses.About 80% of Fibrinogen in organism is distributed in blood plasma and (is about in normal adult 200~400mg/dl), remaining is distributed in tissue.Fibrinogen be containing through disulfide-bonded 3 pairs of polypeptides (a α, b β and γ) the glycoprotein of chain, a α, b β chain is decomposed by thrombin and forms fibrin, thus playing, thrombosis generate, stop blooding blood The Main Function of bolt.Clinically, increase in inflammation, reduce in the hepatic insufficiency of height, dic etc..
The clinical meaning of fibrinogen assay includes but is not limited to: 1. pathologic increases: (1) Pre-thrombosis State and thrombosis Property disease when, body coagulation function strengthens, and plasma fibrinogen increases, such as acute myocardial infarction, diabetes, gestational hypertension Disease, atherosclerosiss, malignant tumor etc..(2) albumen synthesis increases, such as connective tissue disease, multiple myeloma etc..(3) anti- Answering property increases, such as actute infection, acute nephritiss, burn, shock, after major operation etc..2. pathologic reduces: (1) consumes excessively, leads Plasma content is caused to reduce, such as dic etc..(2) Fibrinolytic Activities strengthen, and fib is decomposed, such as constitutional hyperfibrinolysiss disease etc..(3) Synthesis reduces, such as hepatitis gravis, liver cirrhosis etc..
The algoscopy of Fibrinogen includes thrombin additive process (clauss method), Clotting-time method (pt algorithm), exempts from Epidemic disease turbidimetry (tia), emulsion technique etc., typically adopt thrombin additive process.
Under thrombin additive process, the content of Fibrinogen ultimately forms fibre according to Fibrinogen and thrombin action The principle of fibrillarin measures, and makes standard curve with international standard substance for reference blood plasma, during with thrombin to measure the clotting of plasma Between, i.e. thrombin time (thrombin time, tt), gained PCT and fibrinogen concentration in blood plasma are in negative Correlation, thus obtain the content of Fibrinogen.
Specifically, thrombin time refers to add the time of the clotting of plasma after standardized thrombinogen in blood plasma. Under thrombin action, the Fibrinogen in blood plasma to be checked is changed into fibrin.When anticoagulant substanceses in blood plasma to be checked When increasing, thrombin time extends.When blood plasma to be checked be in acid, test object suffers from abnormal fibrous proteinemia situations such as Under, thrombin time shortens.
For example, thrombin time prolongation sees plasma fibrinogen and lowers or textural anomaly;Clinical practice heparin, or Heparin sample anticoagulant substanceses when hepatopathy, nephropathy and systemic lupus erythematosus (sle) increase;Fibrinolytic systemic-function is hyperfunction.
The thrombin using in fibrinogen assay, cuts peptide from the thrombinogen as its precursor and forms tool There is the α-thrombin of coagulation activity.Known this α-thrombin selfdecomposition can become the β without coagulation activity of low-molecular-weight-solidifying Hemase, and then resolve into γ-thrombin, when preserving for a long time, generally carry out lyophilization.
For measuring the reagent of Fibrinogen (fib) content or thrombin time (tt), existing reagent is Freeze-dried reagent, except expensive, in use, is required to redissolve, in-convenience in use, and will necessarily bring and redissolve Cause volumetric errors in journey, lead to result that deviation occurs.And there is not this problem in liquid reagent and easy to use, that is, open Use, difference between batch is less, result is more accurate.Therefore urgently need to develop the stabilizer that can stablize thrombin solution and Stable thrombin solution product.
Content of the invention
The technical problem to be solved is the defect being not easy to preservation for thrombin solution, improves thrombin molten The stability of liquid, thus extending the holding time, reducing and preserving cost, and convenient use reduces experimental error.
Present inventors discovered unexpectedly that gluconic acid radical ion and glutamate ion have stable thrombin molten The cooperative effect of liquid.
The invention provides for the stabilizer of thrombin solution, it comprises Water-Soluble Glucose acid compound and water solublity Glutamic acid compounds.In one embodiment, described stabilizer is by Water-Soluble Glucose acid compound and water solublity glutamic acid Compound forms.In another embodiment, described stabilizer comprises Water-Soluble Glucose acid compound, water solublity glutamic acid Compound and solvent.In another embodiment in addition, described stabilizer comprises Water-Soluble Glucose acid compound, water Dissolubility glutamic acid compounds, solvent and those skilled in the art being capable of conventional use of auxiliary element (such as buffer agents, surface Activating agent, preservative etc.).Described solvent can be that water, organic solvent or those skilled in the art conventional can determine or make One of solvent or two or more combinations.Preferably, described solvent is water.
Preferably, in the stabilizer for thrombin solution of the present invention, Water-Soluble Glucose acid compound and water solublity The ratio of glutamic acid compounds is 1:50 to 50:1.Preferably, the upper limit of described ratio can be 40:1,30:1,20:1,10: 1st, 9:1,8:1,7:1,6:1,5:1,4:1,3:1,2:1, the lower limit of described ratio can be 1:40,1:30,1:20,1:10,1: 9th, 1:8,1:7,1:6,1:5,1:4,1:3,1:2, described ratio can be above-mentioned higher limit and the scope of lower limit combination in any. It is highly preferred that described ratio can be 1:1.
Preferably, described Water-Soluble Glucose acid compound can be Water-Soluble Glucose hydrochlorate.Described water solublity Fructus Vitis viniferae Sugar lime can be one of calcium gluconate, zinc gluconate or magnesium gluconate or two or more combinations.Preferably, Described Water-Soluble Glucose hydrochlorate is calcium gluconate or zinc gluconate.
Water-Soluble Glucose acid compound used in the present invention is commercially available, for example, be derived from Shanghai Aladdin biochemistry section The trade mark of skill limited company (Shanghai Jing Chun biochemical technology limited company) is the gluconic acid of Aladdin (aladdin) Calcium (for example, article No. c110858), the zinc gluconate etc. from lark prestige Science and Technology Ltd..
Preferably, described water solublity glutamic acid compounds can be water-soluble glutamate.It is highly preferred that described water solublity Glutamate, Glu is sodium glutamate, Kaglutam or a combination thereof.Most preferably, described water-soluble glutamate is sodium glutamate.
Water solublity glutamic acid compounds used in the present invention are commercially available, for example, have from Shanghai sky biological reagent The sodium glutamate of limit company, the trade mark from Shanghai Yuan Ye bio tech ltd are Kaglutam (for example, the article No. of source leaf S20427) etc..
Present invention also offers comprising the thrombin solution of the stabilizer of the present invention.
The thrombin solution (referred to as " thrombin solution of the present invention ") that the stabilizer of the present invention is suitable for is to make thrombin It is suspended or dissolved in the mixing of the aqueous solution, organic solvent solution or water and organic solvent in water and/or organic solvent Solution, preferably aqueous solution or water and organic solvent mixed solution.Described organic solvent, as long as do not result in dividing of thrombin Solution and activity suppression etc., and its final use is not affected, just it is not particularly limited, for example dimethyl sulfoxide, glycerol, poly- second Glycol, polypropylene glycol etc..By one of these materials or can also be used in combination.
Preferably, in the thrombin solution of the present invention, calculated with the cumulative volume of thrombin solution, Water-Soluble Glucose is acidified The concentration of compound is 1g/l to 50g/l;It is highly preferred that in the thrombin solution of the present invention, with the total volume meter of thrombin solution Calculate, the concentration of Water-Soluble Glucose acid compound is 2g/l to 40g/l;It is highly preferred that in the thrombin solution of the present invention, with solidifying The cumulative volume of hemase solution calculates, and the concentration of Water-Soluble Glucose acid compound is 3g/l to 30g/l;It is highly preferred that the present invention Thrombin solution in, calculated with the cumulative volume of thrombin solution, the concentration of Water-Soluble Glucose acid compound be 3g/l extremely 25g/l;It is highly preferred that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, Water-Soluble Glucose is acidified The concentration of compound be 2g/l, 3g/l, 4g/l, 5g/l, 6g/l, 7g/l, 8g/l, 9g/l, 10g/l, 15g/l, 20g/l, 25g/l, 30g/l.It is further preferred that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, Water-Soluble Glucose The concentration of acid compound is 7.7g/l.
Preferably, in the thrombin solution of the present invention, calculated with the cumulative volume of thrombin solution, water solublity glutamic acid chemical combination The concentration of thing is 1g/l to 150g/l;It is highly preferred that in the thrombin solution of the present invention, with the total volume meter of thrombin solution Calculate, the concentration of water solublity glutamic acid compounds is 10g/l to 100g/l;It is highly preferred that in the thrombin solution of the present invention, with solidifying The cumulative volume of hemase solution calculates, the concentration of water solublity glutamic acid compounds be 10g/l, 15g/l, 20g/l, 25g/l, 30g/l, 35g/l、40g/l、45g/l、50g/l、55g/l、60g/l、65g/l、70g/l、75g/l、80g/l、85g/l、90g/l、95g/l Or 100g/l;It is further preferred that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, water solublity paddy The concentration of propylhomoserin compound is 50g/l.
The thrombin solution of the present invention can also comprise buffer agent, surfactant and preservative.
Preferably, described buffer agent can be 4- hydroxyethyl piperazine ethanesulfonic acid (n- (2- ethoxy) piperazine-n'-2- ethane Sulfonic acid;Molecular formula: c8h18n2o4s, also known as hepes acid), citric acid, phosphoric acid, acetic acid, imidazoles, 3- (n- morpholine) the third sulphur (mops), two (2- ethoxy) imido grpup three (methylol) methane (bis-tris), trishydroxymethylaminomethane (tris), 3- (n- morpholinyl) -2- hydroxy-propanesulfonic acid (mopso), n- (2- acetylamino)-imino-diacetic acetic acid (ada) or MES One of or two or more combinations (mes);It is highly preferred that buffer agent is 4- hydroxyethyl piperazine ethanesulfonic acid.
Buffer agent used in the present invention is commercially available, for example, be derived from the 4- of Suzhou City Bake bio tech ltd Hydroxyethyl piperazine ethanesulfonic acid, 3- (n- the morpholinyl) -2- hydroxyl third from the uncommon love of ladder (Shanghai) chemical conversion industry Development Co., Ltd Sulfonic acid (for example, product coding h0671), the trade mark from Sa En chemical technology (Shanghai) Co., Ltd. are the 2- morpholine of An Naiji Ethyl sulfonic acid (for example, goods number d090002).
As long as the addition of described buffer agent has the amount of buffer capacity with regard to there is no particular limitation, people in the art Member can the conventional content determining the buffer agent being suitable for using.But, the inventors found that the thrombin of the present invention is molten In liquid, calculated with the cumulative volume of thrombin solution, when the concentration of buffer agent is values below scope, be more beneficial for realizing this Bright purpose: preferably, in the thrombin solution of the present invention, calculated with the cumulative volume of thrombin solution, the concentration of buffer agent is 1g/l to 50g/l;It is highly preferred that in the thrombin solution of the present invention, calculated with the cumulative volume of thrombin solution, buffer agent dense Degree is 5g/l to 24g/l;It is highly preferred that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, buffer agent Concentration be 5.9g/l to 23.8g/l;It is highly preferred that in the thrombin solution of the present invention, with the total volume meter of thrombin solution Calculate, the concentration of buffer agent be 5.9g/l, 6g/l, 7g/l, 8g/l, 9g/l, 10g/l, 11g/l, 11.9g/l, 12g/l, 13g/l, 14g/l, 15g/l, 16g/l, 17g/l, 17.9g/l, 18g/l, 19g/l, 20g/l, 21g/l, 22g/l, 23g/l or 23.8g/l; It is further preferred that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, the concentration of buffer agent is 11.9g/l.
Described surfactant can be anionic surfactant, cationic surfactant, amphion table One of face activating agent or nonionic surfactant or two or more combinations.
Described anionic surfactant can be sodium lauryl sulphate, dodecyl sodium sulfate, dodecyl-n- One of sodium sarcosinate, sodium cholate, NaTDC or sodium taurodeoxycholate or two or more combinations.
Described cationic surfactant can be cetyl trimethylammonium bromide, four decyl ammonium bromide or dodecane One of pyridinum chloride or two or more combinations.
Described zwitterionic surfactant can be 3- [(3- gallbladder amido propyl) Dimethyl Ammonium] -1- propane sulfonic acid salt, 3- [(3- gallbladder amido propyl) Dimethyl Ammonium] -2- hydroxyl -1- propane sulfonic acid salt, palmityl LYSOLECITHIN SUNLECITHIN A, dodecyl-n- glycine betaine Or one of dodecyl-Beta-alanine or two or more combinations.
Described nonionic surfactant can be octyl glucoside, heptyl glucosinolate, capryl-n- methyl Portugal Osamine, polyoxyethylene lauryl ether, polyoxyethylene seven methylhexyl ether, Triton X100, polyoxyethylene nonyl One of base phenyl ether, polyoxyethylene fatty acid ester, sucrose fatty acid ester or polyoxyethylene sorbitol ester or two kinds with On combination.
Preferably, described surfactant is nonionic surfactant;It is highly preferred that described surfactant is poly- Oxygen ethylene Arlacel-80 (also known as Tween 80).
Surfactant used in the present invention is commercially available, for example, be derived from the tween of Chengdu Ke Long chemical reagent factory 80th, be derived from Shanghai Aladdin biochemical technology limited company (Shanghai Jing Chun biochemical technology limited company) trade mark be Ah The Tween 80 (for example, article No. t104866) of Latin (aladdin), the trade mark of Shanghai Yuan Ye bio tech ltd are source leaf Sucrose fatty acid ester (for example, article No. s30894) etc..
As long as the addition of described surfactant makes the stability-enhanced amount of thrombin solution, not especially Limit, those skilled in the art can the conventional content determining the surfactant being suitable for using.But, the present inventor Find, in the thrombin solution of the present invention, to calculate with the cumulative volume of thrombin solution, when the concentration of surfactant is following number During value scope, it is more beneficial for realizing the purpose of the present invention: preferably, calculate with the cumulative volume of thrombin solution, surfactant Concentration be 10 μ l/l to 1000 μ l/l;It is highly preferred that being calculated with the cumulative volume of thrombin solution, the concentration of surfactant is 50 μ l/l to 500 μ l/l;It is highly preferred that being calculated with the cumulative volume of thrombin solution, the concentration of surfactant be 100 μ l/l extremely 400μl/l;It is further preferred that being calculated with the cumulative volume of thrombin solution, the concentration of surfactant is 100 μ l/l, 200 μ L/l, 300 μ l/l or 400 μ l/l;It is further preferred that being calculated with the cumulative volume of thrombin solution, the concentration of surfactant It is 200 μ l/l.
Described preservative can be sodium azide (nan3), Ciprofloxacin, one of propanoic acid or sodium benzoate or two kinds with On combination.Preferably, described preservative is sodium azide.
Preservative used in the present invention is commercially available, for example, come precious biotechnology (Shanghai) limited company westerly Trade mark be the sodium azide (for example, article No. be 0639) of amresco, be derived from Chengdu Hua Xia chemical reagent company limited sodium azide (the brilliant pure biochemical technology share in Shanghai is limited for (for example, article No. is h1100046), Shanghai Aladdin biochemical technology limited company Company) trade mark be the sodium benzoate (for example, article No. be s104128) of Aladdin (aladdin), be derived from Sigma-Aldrich (for example, production code member is the preservative for proclin300 for the trade mark of Co., Ltd (sigma-aldrich llc) 48914-u) etc..
As long as just there is no particular limitation in prescribed limit for the addition of described preservative.Those skilled in the art are permissible The conventional content determining the preservative being suitable for using.But, the inventors found that in the thrombin solution of the present invention, with The cumulative volume of thrombin solution calculates, and when the concentration of preservative is values below scope, is more beneficial for realizing the mesh of the present invention : preferably, calculated with the cumulative volume of thrombin solution, the concentration of preservative is 0.1g/l to 5.0g/l;It is highly preferred that with solidifying The cumulative volume of hemase solution calculates, and the concentration of preservative is 0.2g/l to 2.5g/l;It is highly preferred that it is overall with thrombin solution Long-pending calculating, the concentration of preservative is 0.4g/l to 1.3g/l;It is further preferred that being calculated with the cumulative volume of thrombin solution, prevent The concentration of rotten agent be 0.4g/l, 0.5g/l, 0.6g/l, 0.7g/l, 0.8g/l, 0.9g/l, 1.0g/l, 1.1g/l, 1.2g/l or 1.3g/l;It is further preferred that being calculated with the cumulative volume of thrombin solution, the concentration of preservative is 1.0g/l.
Used in the present invention, thrombin can be the thrombin of the animal origins such as people, pig, cattle, pass through genetic engineering legal system Standby thrombin or commercially available medicine.Thrombin used in the present invention is commercially available, is e.g. derived from Hunan one lattice pharmacy The thrombin lyophilized powder of company limited, coagulating from Sigma-Aldrich Co., Ltd (sigma-aldrich llc) Hemase preparation (for example, production code member is 10602400001) etc..
As long as it is just not special that the addition of the thrombin in the thrombin solution of the present invention is suitable for the purpose of the present invention Limit.It was found by the inventors of the present invention that in the thrombin solution of the present invention, being calculated with the cumulative volume of thrombin solution, thrombin Concentration can be 1ku/l to 120ku/l;It is highly preferred that in the thrombin solution of the present invention, with the cumulative volume of thrombin solution Calculate, the concentration of thrombin can be 1ku/l, 2ku/l, 3ku/l, 4ku/l, 5ku/l, 6ku/l, 7ku/l, 8ku/l, 9ku/l, 10ku/l、20ku/l、30ku/l、40ku/l、50ku/l、60ku/l、70ku/l、80ku/l、90ku/l、100ku/l、110ku/ L or 120ku/l;It is highly preferred that in the thrombin solution of the present invention, calculated with the cumulative volume of thrombin solution, thrombin dense Degree can be 2ku/l to 110ku/l, 5ku/l to 100ku/l, 10ku/l to 90ku/l, 15ku/l to 80ku/l, 20ku/l extremely 70ku/l, 25ku/l to 60ku/l, 30ku/l to 50ku/l;It is further preferred that in the thrombin solution of the present invention, with blood coagulation The cumulative volume of enzymatic solution calculates, and the concentration of thrombin can be 2ku/l, 4ku/l, 30ku/l, 70ku/l, 120ku/l.
Preferably, the thrombin solution of the present invention, is calculated with the cumulative volume of thrombin solution, comprising concentration is 7.7g/l Calcium gluconate, concentration are the sodium glutamate of 50g/l, concentration is that the 4- hydroxyethyl piperazine ethanesulfonic acid of 11.9g/l, concentration are The sodium azide of 1.0g/l, concentration are the polyoxyethylene sorbitan monooleate dehydration of 200 μ l/l.It is highly preferred that above-mentioned thrombin In solution, comprise the thrombin that concentration is 2ku/l, 4ku/l, 30ku/l or 70ku/l.
Preferably, the thrombin solution of the present invention, is calculated with the cumulative volume of thrombin solution, comprising concentration is 7.7g/l Zinc gluconate, concentration are the sodium glutamate of 50g/l, concentration is that the 4- hydroxyethyl piperazine ethanesulfonic acid of 11.9g/l, concentration are The sodium azide of 1.0g/l, concentration are the polyoxyethylene sorbitan monooleate dehydration of 200 μ l/l.It is highly preferred that above-mentioned thrombin In solution, comprise the thrombin that concentration is 2ku/l, 4ku/l, 30ku/l or 70ku/l.
Present invention also offers the method preparing thrombin solution, methods described includes the step of the stabilizer using the present invention Suddenly.
Present invention also offers the stabilizer of the present invention is used for improving the purposes of thrombin solution stability.
Present invention also offers the thrombin solution of the stabilizer of the present invention or the present invention is used for the purposes of reagent preparation.
Present invention also offers a kind of reagent, it contains the thrombin solution of the stabilizer of the present invention or the present invention.
Stabilizer or the reagent of thrombin solution preparation of the present invention or stablizing containing the present invention using the present invention The reagent of the thrombin solution of agent or the present invention can be referred to as the reagent of the present invention.
Preferably, described reagent is the reagent for detection fibers proteinogen or thrombin time.
Preferably for the present invention for detection fibers proteinogen reagent, the containing of the thrombin in thrombin solution Measure as 30ku/l or 70ku/l;Thrombin for the present invention for detecting the reagent of thrombin time, in thrombin solution Content be 2ku/l or 4ku/l.
Present invention also offers a kind of test kit, it comprises the reagent of the present invention.
The present inventors have noted that, in the case that thrombin solution other components are constant, under different concentration of thrombin, contain The measured value having the reagent of the thrombin solution of the present invention can overall improve, but this is to the thrombin solution of the present invention and correlation The purposes of the stability of product itself and correlation, the enforcement of method do not have an impact, and the raising of measured value also will not hinder this The realization of the function of bright thrombin solution and Related product.In order to obtain the measured value in ideal range, people in the art Member can conventional adjustment thrombin content realizing above-mentioned target.
The thrombin solution convenient use of the stabilizer containing the present invention, need not redissolve, it is to avoid due to redissolving volume difference Lead to error.Plug and play, difference between batch is less, and result is more accurate.
Thrombin solution stability using the stabilizer preparation of the present invention is strong, stablizes more than 1 year for 2-8 DEG C, 37 DEG C stable More than 20 days, 2-8 DEG C opened stability more than 10 days.Thus, the stabilizer of the present invention can improve stablizing of thrombin solution Property, improve storage form and the condition of Related product, reduce the cost producing and applying.
Specific embodiment
Used in the following examples of the present invention, each Component Source is respectively as follows: from Shanghai Aladdin biochemical technology share The trade mark of company limited (Shanghai Jing Chun biochemical technology limited company) is the calcium gluconate (example of Aladdin (aladdin) As article No. c110858), from lark prestige Science and Technology Ltd. zinc gluconate, be derived from the limited public affairs of Shanghai source leaf biotechnology The trade mark of department is the Kaglutam (for example, article No. s20427) of source leaf, the sodium glutamate of Shanghai sky biological reagent company limited, The 4- hydroxyethyl piperazine ethanesulfonic acid (hepes acid) of Suzhou City Bake bio tech ltd, Chengdu Ke Long chemical reagent factory Tween 80, the trade mark of west treasured biotechnology (Shanghai) limited company are the sodium azide (article No. 0639) of amresco, Hunan one The thrombin lyophilized powder of lattice pharmaceutical Co. Ltd.
Embodiment 1
The preparation of thrombin time (tt) detectable of the stabilizer containing the present invention
Weigh hepes acid 11.9g, calcium gluconate 7.7g, sodium glutamate 50g, sodium azide 1g, Tween 80 0.2g, add Dissolve in distilled water, adjust ph to 6.4 with sodium hydroxide, be settled to 1l.Take thrombin 2 (2000u/ props up), prepared with above Buffer 1ml/ props up dissolving, takes dissolving thrombin 3.6ml (scalable enzyme amount controls difference between batch), adds in 1l buffer and shake up, Tt detectable is prepared and is completed.
Product performance index
1. repeatability: the coefficient of variation (cv)≤5%;With normal Quality Control blood plasma retest 10 times, calculate measure average ValueWith standard deviation (s).Calculate the coefficient of variation (cv) according to formula (1).Acquired results should meet wanting of following 3. stability Ask.
c v ( % ) = s x &overbar; × 100... ( 1 )
In formula:
In s: standard deviation
Measure average
2. difference between batch: the coefficient of variation (cv)≤10%;Test the reagent of 3 different batches with normal Quality Control blood plasma respectively, Each batch measures retest 10 times, calculates 30 measured value meansigma methodssWith standard deviation (s), calculate according to formula (1) The coefficient of variation (cv).
3. stability
2 DEG C~8 DEG C airtight preservations of this product, are newly opened one bottle of mensure Quality Control blood plasma every time, were contrasted with first day, relative deviation exists In 15%, 12 months effect duration.
Embodiment 2
The detection method of thrombin time (tt) detectable
Take blood plasma 100 μ l, 37 DEG C preheat 2 minutes, are subsequently adding thrombin reagent 100 μ l, in ca550 full automatic blood-coagulation instrument (producer sysmex) measures according to the description of producer.
Points for attention:
1. blood sampling should avoid haemolysis, prevents tissue fluid to be mixed into.Will smoothly during blood drawing, anticoagulant fully will can not have sludged blood; Platelet must be removed during separated plasma.
2. anticoagulant should not be made with edta and heparin during sample collection.The ratio of blood and anticoagulant should accurately, blood sampling volume The specimen that deviation is more than 10% should not use.
If 3. hematocrit≤20% or >=55%, need to adjust the ratio of blood sample and anticoagulant, anticoagulant milliliter number =0.00185 × blood milliliter number × (100- hematocrit).
4. use calibrated after measuring pipette and sample injector.
5. use the plastics of cleanliness without any pollution or the glass drying oven of silication.
6. experimental temperature controls at 37 DEG C ± 1.0 DEG C.
7. reagent and sample size can change as needed in proportion.
8. reagent, using finishing, should be wiped clean bottleneck, screw bottle cap as early as possible, put back in time and protect under the condition of storage of requirement Deposit.
Embodiment 3
The preparation of Fibrinogen (fib) detectable of the stabilizer containing the present invention
(1) reagent preparation: weigh hepes acid 11.9g, calcium gluconate 7.7g, sodium glutamate 50g, sodium azide 1g, tell Warm 80 0.2g, add in distilled water and dissolve, and adjust ph to 6.4 with sodium hydroxide, are settled to 1l.Take 30 (3000u/ of thrombin ), prop up dissolving with the above buffer 1ml/ for preparing, all add in 1l buffer and shake up, fib detectable is prepared and completed.
(2) prepared and diluted sample buffer: weigh imidazoles 3.06g, sodium chloride 5.22g, sodium citrate 1.2g, sodium azide 0.95g, adds in distilled water and dissolves, and adjusts ph to 7.30 with sodium hydroxide, is settled to 1l.After stable in two days, adjust ph again To 7.30.
Product performance index
1. accuracy: take reference material or the test of accurateness Quality Control thing, in triplicate, obtain meansigma methodss, according to formula (2) Calculate the relative deviation of meansigma methodss and reference material or main calibration object, result should meet relative deviation should be in the range of ± 15% Require.Computing formula:
(computing formula: material or main calibration object relatively inclined Difference ... ... ... (2)
In formula:
X --- detection average;
Xc --- reference material or accurateness Quality Control thing sign value.
2. repeatability
Distinguish retest 10 times with normal Quality Control blood plasma and abnormal Quality Control blood plasma, and calculate the meansigma methodss of mensureWith Standard deviation (s).Calculate the coefficient of variation (cv) by formula (1), result should meet the requirement of the coefficient of variation (cv)≤8%.
3. difference between batch
Test the reagent of 3 different batches with normal Quality Control blood plasma, each batch is tested 10 times, calculate 30 measured values and put down AverageWith standard deviation (s), calculate the coefficient of variation (cv) according to formula (1), result should meet the coefficient of variation (cv)≤15% Requirement.
4. stability
2 DEG C~8 DEG C airtight preservations of this product, newly open every time one bottle mensure Quality Control blood plasma, relative deviation in 15%, effect duration 12 months.
Embodiment 4
The detection method of Fibrinogen (fib) detectable
(1) standard curve is set up
Dilute reference blood plasma with diluent according to the form below, you can acquisition series concentration:
Take fib detectable pre-temperature 3 minutes, to 37 DEG C.Take the reference blood plasma after dilution 100 μ l, 37 DEG C of pre-temperatures 2 minutes. Add 50 μ l pre-temperature reagent, mix at once and timing, record setting time.With the obtained target level of reference blood plasma gradient dilution it is Abscissa, corresponding setting time (second) is vertical coordinate, and measurement result is mapped on double logarithmic curve, or input instrument is according to corresponding Mathematical model automatically generate working curve.
(2) sample measures
Sample dilution buffer carries out 10 times of dilutions, and determination step is with the preparation of working curve.Automatically coagulated with ca550 Blood instrument (producer sysmex) measures according to the description of producer.
Points for attention:
1. blood sampling should avoid haemolysis, prevents tissue fluid to be mixed into.Will smoothly during blood drawing, anticoagulant fully will can not have sludged blood; Platelet must be removed during separated plasma.
2. anticoagulant should not be made with edta and heparin during sample collection.The ratio of blood and anticoagulant should accurately, blood sampling volume The specimen that deviation is more than 10% should not use.
If 3. hematocrit≤20% or >=55%, need to adjust the ratio of blood sample and anticoagulant, anticoagulant milliliter number =0.00185 × blood milliliter number × (100- hematocrit).
4. use calibrated after measuring pipette and sample injector.
5. use the plastics of cleanliness without any pollution or the glass drying oven of silication.
6. experimental temperature controls at 37 DEG C ± 1.0 DEG C.
7. reagent and sample size can change as needed in proportion.
8. reagent, using finishing, should be wiped clean bottleneck, screw bottle cap as early as possible, put back in time and protect under the condition of storage of requirement Deposit.
Embodiment 5
Exist between Water-Soluble Glucose acid compound and water solublity glutamic acid compounds and stablize the collaborative of thrombin solution Effect
Under conditions of its dependent variable is consistent, for containing only calcium gluconate, contain only sodium glutamate, contain Portugal simultaneously Grape Calciofon and sodium glutamate and at four kinds of thrombin solutions containing calcium gluconate and Kaglutam measure 37 DEG C simultaneously Stabilization time, with relative deviation 10% as nature controlling line, observe above-mentioned thrombin solution testing result.Testing result takes 5 times The average of test.
In table 1, the content of each composition of thrombin solution is respectively as follows: calcium gluconate 7.7g/l (such as containing), sodium glutamate 50g/l (such as containing), Kaglutam 50g/l (such as containing), hepes acid 11.9g/l, sodium azide 1g/l, Tween 80 200 μ l/l, Thrombin 2ku/l.
Table 1: calcium gluconate and water solublity glutamic acid compounds stablize the cooperative effect of thrombin solution
Table 2 calcium gluconate and water solublity glutamic acid compounds stablize the test of thrombin solution
From table 1, table 2 it is observed that calcium gluconate and water solublity glutamic acid compounds simultaneously in the presence of, thrombin is molten The stable natural law of liquid is the longest.Therefore, exist between calcium gluconate and water solublity glutamic acid compounds and stablize thrombin solution Cooperative effect.
The present invention also have chosen the thrombin solution containing zinc gluconate and sodium glutamate to verify water solublity further There is the cooperative effect stablizing thrombin solution between gluconic acid compound and water solublity glutamic acid compounds.At measuring 37 DEG C Stabilization time, with relative deviation 10% as nature controlling line, observe above-mentioned thrombin solution testing result.Testing result takes 3 times The average of test.
Above-mentioned zinc gluconate and sodium glutamate containing as composition each in the thrombin solution of stabilizer as stabilizer Amount is respectively as follows: zinc gluconate 7.7g/l, sodium glutamate 50g/l, hepes acid 11.9g/l, sodium azide 1g/l, Tween 80 200 μ L/l, thrombin 30ku/l (fib reagent) or 2ku/l (tt reagent).The stability test of above-mentioned thrombin solution is as follows.
Table 3 zinc gluconate and sodium glutamate stablize the test of thrombin solution
Good synergisticing stable effect is also had by the visible zinc gluconate of table 3 and sodium glutamate.
Therefore, can be seen that between Water-Soluble Glucose acid compound and water solublity glutamic acid compounds from above-mentioned experiment There is the cooperative effect stablizing thrombin solution.
Embodiment 6
The stablizing effect to thrombin solution for the aminoacid or its salt of calcium gluconate and other non-glutamic acids
In thrombin solution the content of each composition be respectively as follows: calcium gluconate 7.7g/l, glycine 50g/l (such as containing), Arginine 50g/l (such as containing), serine 50g/l (such as containing), glutamic acid 50g/l (such as containing), hepes acid 11.9g/l, folded Nitrogen sodium 1g/l, Tween 80 200 μ l/l.Thrombin is 2ku/l.
With relative deviation 10% as nature controlling line, according to the experimental result of table 4,5 in table 1 in embodiment 5 and the present embodiment, It is molten to thrombin that the aminoacid of calcium gluconate and other non-glutamic acids or its salt do not enable water solublity glutamic acid compounds The stablizing effect of liquid.
Table 4: the aminoacid of calcium gluconate and other non-glutamic acids stablizes the cooperative effect of thrombin solution
Table 5: calcium gluconate stablizes the cooperative effect of thrombin solution with glycine or L-Valine
In embodiment 7-11, in thrombin solution during a certain component content change, the content of other compositions follows following number Value: calcium gluconate 7.7g/l, sodium glutamate 50g/l, hepes acid 11.9g/l, sodium azide 1g/l, Tween 80 200 μ l/l.Close The content of enzyme in thrombin solution, in tt reagent, the content of enzyme is 2ku/l;In fib reagent, the content of enzyme is 30ku/l.
Embodiment 7
The content range of hepes acid in thrombin solution
According to table 6, with 15% as nature controlling line, in thrombin solution hepes acid content range can be 5.9g/l extremely 23.8g/l.
The content range of hepes acid in table 6 thrombin solution
Embodiment 8
The content range of calcium gluconate in thrombin solution
According to table 7, with 15% as nature controlling line, in thrombin solution the content range of calcium gluconate can be 3g/l extremely 25g/l.
The content range of calcium gluconate in table 7 thrombin solution
Embodiment 9
The content range of thrombin solution Glutamic Acid sodium
According to table 8, with 15% as nature controlling line, the content range of thrombin solution Glutamic Acid sodium can be 10g/l extremely 100g/l.
The content range of table 8 thrombin solution Glutamic Acid sodium
Embodiment 10
The content range of sodium azide in thrombin solution
According to table 9, with 15% as nature controlling line, in thrombin solution the content range of sodium azide can be 0.4g/l extremely 1.3g/l.
The content range of sodium azide in table 9 thrombin solution
Embodiment 11
The content range of Tween 80 in thrombin solution
According to table 10, with 15% as nature controlling line, in thrombin solution the content range of Tween 80 can be 100 μ l/l extremely 400μl/l.
The content range of Tween 80 in table 10 thrombin solution

Claims (21)

1. a kind of thrombin solution, it comprises stabilizer, and wherein said stabilizer comprises Water-Soluble Glucose acid compound and water Dissolubility glutamic acid compounds.
2. thrombin solution according to claim 1, wherein said Water-Soluble Glucose acid compound and described water solublity paddy ammonia The ratio of acid compound is 1:50 to 50:1.
3. the thrombin solution according to claim 1 or 2, wherein said Water-Soluble Glucose acid compound is Water-Soluble Glucose Hydrochlorate.
4. thrombin solution according to claim 3, wherein said Water-Soluble Glucose hydrochlorate is calcium gluconate, gluconic acid One of zinc or magnesium gluconate or two or more combinations.
5. the thrombin solution according to claim 1 or 2, wherein said water solublity glutamic acid compounds are water solublity glutamic acid Salt.
6. thrombin solution according to claim 5, wherein said water-soluble glutamate be sodium glutamate, Kaglutam or its Combination.
7. thrombin solution according to claim 1, is wherein calculated with the cumulative volume of thrombin solution, and Water-Soluble Glucose is acidified The concentration of compound is 1g/l to 20g/l.
8. thrombin solution according to claim 1, is wherein calculated with the cumulative volume of thrombin solution, water solublity glutamic acid chemical combination The concentration of thing is 1g/l to 150g/l.
9., according to the thrombin solution in claim 1, it also comprises buffer agent, surfactant and preservative.
10. thrombin solution according to claim 9, wherein said buffer agent is 4- hydroxyethyl piperazine ethanesulfonic acid, citric acid, phosphorus Acid, acetic acid, imidazoles, 3- (n- morpholine) the third sulphur, two (2- ethoxy) imido grpup three (methylol) methane, trihydroxy methyl amino first In alkane, 3- (n- morpholinyl) -2- hydroxy-propanesulfonic acid, n- (2- acetylamino)-imino-diacetic acetic acid or MES one Plant or two or more combinations.
11. thrombin solutions according to claim 9, wherein said surfactant be anionic surfactant, sun from One of sub- property surfactant, zwitterionic surfactant or nonionic surfactant or two or more groups Close.
12. thrombin solutions according to claim 11, wherein said anionic surfactant be sodium lauryl sulphate, One of dodecyl sodium sulfate, dodecyl-n- sodium sarcosinate, sodium cholate, NaTDC or sodium taurodeoxycholate Or two or more combinations.
13. thrombin solutions according to claim 11, wherein said cationic surfactant is cetyl trimethyl One of ammonium bromide, four decyl ammonium bromide or dodecanyl pyridinium chloride or two or more combinations.
14. thrombin solutions according to claim 11, wherein said zwitterionic surfactant is 3- [(3- gallbladder amide third Base) Dimethyl Ammonium] -1- propane sulfonic acid salt, 3- [(3- gallbladder amido propyl) Dimethyl Ammonium] -2- hydroxyl -1- propane sulfonic acid salt, palmityl be molten One of blood lecithin or dodecyl-n- glycine betaine or dodecyl-Beta-alanine or two or more combinations.
15. thrombin solutions according to claim 11, wherein said nonionic surfactant is octyl glucoside, heptyl Glucosinolate, capryl-n- methylglucosamine, polyoxyethylene lauryl ether, polyoxyethylene seven methylhexyl ether, polyoxy second Alkene isooctyl phenyl ether, ethylene nonyl phenyl ether, polyoxyethylene fatty acid ester, sucrose fatty acid ester or poly(ethylene oxide) mountain One of pears sugar alcohol ester or two or more combinations.
16. thrombin solutions according to claim 9, wherein said preservative is sodium azide, Ciprofloxacin, propanoic acid or benzoic acid One of sodium or two or more combinations.
A kind of 17. reagent, comprise the thrombin solution according to any one of claim 1 to 16.
18. reagent according to claim 17, it is the reagent for detection fibers proteinogen or thrombin time.
A kind of 19. test kits, it comprises the reagent according to claim 17 or 18.
A kind of 20. methods of detection fibers proteinogen, including using the thrombin solution according to any one of claim 1 to 16 Or the step using the reagent according to claim 17 or 18.
A kind of 21. methods of detection thrombin time, including using the thrombin solution according to any one of claim 1 to 16 Or the step using the reagent according to claim 17 or 18.
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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN109239373A (en) * 2018-08-15 2019-01-18 迪瑞医疗科技股份有限公司 A kind of tissue factor carboxylate reagent and the preparation method and application thereof

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EP0302754B1 (en) * 1987-08-05 1993-11-03 Green Cross Corporation Stable aqueous thrombin solution
CN101305093A (en) * 2005-11-11 2008-11-12 东洋纺织株式会社 Method for stabilization of biological molecule and composition
CN101558310A (en) * 2006-12-21 2009-10-14 积水医疗株式会社 Method for stabilizing a-thrombin in thrombin-containing solution
CN105925545A (en) * 2008-04-21 2016-09-07 诺沃—诺迪斯克保健股份有限公司 Dry Transglutaminase Composition

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EP0302754B1 (en) * 1987-08-05 1993-11-03 Green Cross Corporation Stable aqueous thrombin solution
CN101305093A (en) * 2005-11-11 2008-11-12 东洋纺织株式会社 Method for stabilization of biological molecule and composition
CN101558310A (en) * 2006-12-21 2009-10-14 积水医疗株式会社 Method for stabilizing a-thrombin in thrombin-containing solution
CN105925545A (en) * 2008-04-21 2016-09-07 诺沃—诺迪斯克保健股份有限公司 Dry Transglutaminase Composition

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN109239373A (en) * 2018-08-15 2019-01-18 迪瑞医疗科技股份有限公司 A kind of tissue factor carboxylate reagent and the preparation method and application thereof

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