CN107356765A - A kind of immunoglobulin E detection kit and detection method - Google Patents

A kind of immunoglobulin E detection kit and detection method Download PDF

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Publication number
CN107356765A
CN107356765A CN201710681037.9A CN201710681037A CN107356765A CN 107356765 A CN107356765 A CN 107356765A CN 201710681037 A CN201710681037 A CN 201710681037A CN 107356765 A CN107356765 A CN 107356765A
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reagent
immunoglobulin
preservative
buffer solution
nonidet
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CN107356765B (en
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耿英利
罗湘宇
甘萍萍
黎明
龙腾镶
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Mike Biological Ltd By Share Ltd
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Mike Biological Ltd By Share Ltd
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    • GPHYSICS
    • 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
    • G01N33/68Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving proteins, peptides or amino acids
    • G01N33/6854Immunoglobulins

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  • Health & Medical Sciences (AREA)
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  • Hematology (AREA)
  • Food Science & Technology (AREA)
  • Proteomics, Peptides & Aminoacids (AREA)
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Abstract

The present invention provides a kind of Immunoturbidimetric kit, and it includes reagent R1 and reagent R2, and Nonidet P40 is included in wherein reagent R1, Nonidet P40, magnesium salts, calcium acetate and antibody are included in reagent R2.Kit antibody performance of the invention is good, reproducible, reagent testing result is accurate, disclosure satisfy that requirement.

Description

A kind of immunoglobulin E detection kit and detection method
Technical field
The present invention relates to medical immunology in-vitro diagnosis field, and in particular to a kind of immunoglobulin E detection kit and inspection Survey method.
Background technology
Turbidimetry is widely used in clinical examination work.It is immunoturbidimetry that application is most common now.
It is all by observing the formation of sediment, aggegation and the generation of haemolysis that the immuno analytical method of early stage is most of The presence or absence of specific protein and content in testing sample are analyzed in the light scattering caused by aggregate with measure, such as immune to expand Scattered, immunoelectrophoresis, direct and brief introduction blood clotting, passive hemagglutination, complement fixation test etc., these detection method costs are low, result is easy In judgement, technically it is easy to grasp, can be widely used for detecting polytype clinical sample.But because above method operation is numerous It is trivial, time-consuming and sensitivity and poor accuracy and tend to be eliminated.
Immunoturbidimetry overcomes disadvantages mentioned above, and quantitatively accurate automation can be developed with reference to the demand of clinic Instrument.Therefore, for immunology detection, immunoturbidimetry has immunology antigen, the specificity of antibody binding, has again Biotrepy feature, during body fluid can be detected in automation biochemical instruments, the micro test substance particularly in blood, It is a kind of clinical examination practical technique having very much using future.
Immunoturbidimetry (Turbidimetric inhibition immuno assay) is that antigen-antibody combines dynamic survey Determine method.Its general principle is:When antigen and antibody react and suitable (the general provision antibody of ratio in special dilution system It is excessive) when, in the presence of the poly- agent of rush of the soluble immune complex of formation in dilution system, separate out, formed micro- from liquid phase Grain, makes reaction solution turbidity occur.When antibody concentration is fixed, the amount of the immune complex of formation is with the increasing of amount of antigen in sample Add and increase, the turbidity of reaction solution is consequently increased.Compareed by the turbidity for determining reaction solution with series of standards product, you can meter Calculate the content of antigen in sample.
The various detecting instruments developed according to the general principle of immunoturbidimetry, developed have been widely used in clinical inspection The many aspects tested, it is the basic functional principle of Blood coagulation instrument optical method and immunization;It is the load fat in full-automatic biochemical measure Albumen, haptens and other protein measuring principles;It can also be applied to microorganism detection simultaneously.By accurately to more Kind material is quantified, and the diagnosis, treatment and prognosis evaluation to many diseases have larger clinical meaning.
The conventional immunoturbidimetry of clinic because its sample dosage is few, can directly on automatic clinical chemistry analyzer batch sample Analyze, be simple to operate, but the reagent and method established at present all have some shortcoming and defect, are mainly manifested in:
Antibody is easy to cotton-shaped or flaky precipitate occur during preservation, cause antibody performance be deteriorated, repeatability it is bad, The coefficient of variation (CV) becomes big, directly contributes reagent testing result inaccuracy, and increases filtration step, complex operation, and filters Antibody may be removed, influences Detection results, patient is affected, it is impossible to meets requirement.
The content of the invention
To solve the above problems, the invention discloses a kind of immunoglobulin E detection kit and detection method, reagent are steady It is qualitative it is good, homogeneity is good, testing result accuracy is good, easy to operate, easy to utilize.
For achieving the above object, the present invention provides following technical scheme:
We's invention provides a kind of immunoglobulin E detection kit, wherein including reagent R1 and reagent R2, the examination Included in agent R1 in Nonidet P40 0.9-50g/L, the reagent R2 and include Nonidet P40 0.9-50g/ L, magnesium salts 0.01-15g/L, calcium acetate 0.01-20.5g/L and antibody 10-1000mg/L.
A kind of immunoglobulin E detection kit, Nonidet P40 is 4.5-42g/L in the reagent R1, excellent Elect 33g/L as;Nonidet P40 is 5-42g/L, preferably 29g/L in the reagent R2.
A kind of immunoglobulin E detection kit, the magnesium salts are 0.05-10g/L, preferably 7g/L;The magnesium salts is excellent Elect the one or more in magnesium sulfate, magnesium chloride or magnesium acetate as.
A kind of immunoglobulin E detection kit, the calcium acetate are 0.05-15g/L, preferably 12g/L.
Wherein,
Buffer solution, inorganic salts, preservative and aggregation are also included in the reagent R1;Preferably, in the reagent R1 also Include buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L and aggregation 1-60g/L.
Buffer solution, inorganic salts and preservative are also included in the reagent R2, it is preferable that also comprising buffering in the reagent R2 Liquid 20-100mmol/L, inorganic salts 1-30g/L and preservative 0.5-1g/L.
A kind of immunoglobulin E detection kit, wherein also including calibration object, the calibration object is calibrated using multiple spot, institute State calibration object include buffer solution 20-100mmol/L, inorganic salts 1-30g/L, preservative 0.1-2g/L, glucan 0.3-100g/L, Trehalose 1-100g/L, sucrose 1-100g/L, bovine serum albumin(BSA) 1-100g/L and antigen.
A kind of immunoglobulin E detection kit, wherein being buffered comprising being included in reagent R1 and reagent R2, the reagent R1 Liquid 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, Macrogol 6000 1-60g/L, the poly- second of ethylphenyl Buffer solution 20-100mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/ are included in glycol 0.9-50g/L, the reagent R2 L, antibody 10-1000mg/L, Nonidet P40 0.9-50g/L, magnesium sulfate 0.01-15g/L, calcium acetate 0.01- 20.5g/L;
Preferably,
Buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, poly- second are included in the reagent R1 Buffer solution 20-100mmol/ is included in the 1-60g/L of glycol 6000, Nonidet P40 4.5-42g/L, the reagent R2 L, inorganic salts 1-30g/L, preservative 0.5-1g/L, antibody 10-1000mg/L, Nonidet P40 5-42g/L, magnesium sulfate 0.05-10g/L, calcium acetate 0.05-15g/L;
It is highly preferred that
Buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, poly- second are included in the reagent R1 Buffer solution 20-100mmol/L, nothing are included in the 1-60g/L of glycol 6000, Nonidet P40 33g/L, the reagent R2 Machine salt 1-30g/L, preservative 0.5-1g/L, antibody 10-1000mg/L, Nonidet P40 29g/L, magnesium sulfate 7g/L, Calcium acetate 12g/L.
A kind of immunoglobulin E detection kit,
Preferably, the antibody is goat-anti people, rabbit-anti people, horse is anti-human, mouse is anti-human or other animal anti-human antibodies;
Preferably, the buffer solution be acetate buffer, ammonium chloride buffer, phosphate buffer, TRIS buffer solutions, One or more in borate buffer, glycine buffer, CAPSO, MOPS or Hepes buffer solution;
Preferably, the inorganic salts are one or both of sodium chloride, potassium chloride;
Preferably, the preservative is Sodium azide, phenol, P-hydroxybenzoic acid, ethyl-para-hydroxybenzoate or ethyl mercury One or more in sodium thiosulfate;
Preferably, the aggregation is polyethylene glycol 2000, Macrogol 4000, Macrogol 6000 or polyethylene glycol One or more in 8000;
Present aspect additionally provides a kind of detection method using above-mentioned immunoglobulin E detection kit, including following step Suddenly:
(1) add reagent R1 into testing sample to mix, testing sample and reagent R1 are (1-9) by volume:300 add Enter, 37 DEG C of incubations, under certain wavelength, read absorbance A 1;
(2) add reagent R2 into the mixed liquor of step (1) to mix, reagent R2 and reagent R1 is 1 by volume:(1-6) Add, 37 DEG C of incubations, under certain wavelength, read absorbance A 2;
(3) absorbance △ A, △ A=A2-A1 are drawn;
(4) built-in curve matching model fitting standard curve, root are passed through on automatic clinical chemistry analyzer using calibration object Calculate the content of immunoglobulin E in testing sample automatically according to absorbance.
Signified aggregation is the material for promoting antigen-antibody aggegation in the reaction in the present invention.
It is as follows to be related to raw material sources in present invention offer immunoglobulin E detection kit and detection method:
By adopting the above-described technical solution, the beneficial effects of the invention are as follows:
Immunoglobulin E detection kit and detection method provided by the invention, reagent stability is good, and homogeneity is good, resists Body, which can be stablized, to be preserved, and is not in deposited phenomenon, and antibody titer is high, performance is good, and does not have filtration step, easy to operate, Cost is cheap, and testing result is accurate, reproducible, has wider versatility.
Embodiment
In order that those skilled in the art more fully understand the technical scheme in the application, with reference to embodiment to this hair It is bright to be described further, it is clear that described embodiment is only some embodiments of the present application, rather than whole implementation Example.Based on the embodiment in the application, what those of ordinary skill in the art were obtained under the premise of creative work is not made Every other embodiment, it should all belong to the scope of the application protection.
The immunoglobulin E detection kit of embodiment 1
Reagent R1:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Macrogol 6000 1g/L
Nonidet P40 0.9g/L
Reagent R2:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Goat anti-human immunoglobulin's E antibody 10mg/L
Nonidet P40 0.9g/L
Magnesium sulfate 0.01g/L
Calcium acetate 0.01g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (20mmol/L phosphate buffers, 2g/L sodium chloride, 0.2g/L Sodium azide, 0.3g/L glucans, 1g/L trehaloses, 2g/L sucrose, 2g/L bovine serum albumin(BSA)s) dissolving, with commercially available contrast agents Detect and adjust to 120mg/L, packing and be stored in -20 DEG C.Various concentrations are diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (immunoglobulin E antigen concentration:0mg/L、10mg/L、20mg/L、50mg/L、70mg/L).So Membrane filtration afterwards with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 2
Reagent R1:
Phosphate buffer 40mmol/L
Potassium chloride 7g/L
Phenol 0.7g/L
Macrogol 6000 30g/L
Nonidet P40 50g/L
Reagent R2:
Phosphate buffer 40mmol/L
Potassium chloride 5g/L
Phenol 0.7g/L
Goat anti-human immunoglobulin's E antibody 50mg/L
Nonidet P40 50g/L
Magnesium sulfate 15g/L
Calcium acetate 20.5g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (50mmol/L glycine buffers, 10g/L sodium chloride, 0.5g/L Sodium azide, 20g/L glucans, 25g/L trehaloses, 30g/L sucrose, 20g/L bovine serum albumin(BSA)s) dissolving, is tried with commercially available control Agent, which is detected and adjusted to 100mg/L, packing, is stored in -20 DEG C.Using preceding taking-up, and it is diluted to standard dilutions different dense Immunoglobulin E standard items (the immunoglobulin E antigen concentration of degree:0mg/L、10mg/L、30mg/L、50mg/L、70mg/L). Then the membrane filtration with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 3
Reagent R1:
Acetate buffer 80mmol/L
Potassium chloride 20g/L
Sodium azide 0.8g/L
Macrogol 6000 45g/L
Nonidet P40 4.5g/L
Reagent R2:
Acetate buffer 80mmol/L
Potassium chloride 20g/L
Sodium azide 1g/L
Goat anti-human immunoglobulin's E antibody 300mg/L
Nonidet P40 5g/L
Magnesium sulfate 0.05g/L
Calcium acetate 0.05g/L
Calibration object:
With standard dilutions, (70mmol/L TRIS buffer solutions, 25g/L sodium chloride, 1g/L are folded immunoglobulin E antigen Nitrogen sodium, 55g/L glucans, 50g/L trehaloses, 60g/L sucrose, 75g/L bovine serum albumin(BSA)s) dissolving, with commercially available contrast agents Detect and adjust to 200mg/L, packing and be stored in -20 DEG C.Various concentrations are diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (immunoglobulin E antigen concentration:2mg/L、10mg/L、40mg/L、60mg/L、80mg/L).So Membrane filtration afterwards with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 4
Reagent R1:
MOPS buffer solutions 150mmol/L
Sodium chloride 30g/L
Sodium azide 1g/L
Macrogol 6000 55g/L
Nonidet P40 42g/L
Reagent R2:
MOPS buffer solutions 100mmol/L
Sodium chloride 30g/L
Sodium azide 1g/L
Goat anti-human immunoglobulin's E antibody 600mg/L
Nonidet P40 42g/L
Magnesium sulfate 10g/L
Calcium acetate 15g/L
Calibration object:
With standard dilutions, (100mmol/L TRIS buffer solutions, 15g/L sodium chloride, 1g/L are folded immunoglobulin E antigen Nitrogen sodium, 10g/L glucans, 100g/L trehaloses, 95g/L sucrose, 100g/L bovine serum albumin(BSA)s) dissolving, is tried with commercially available control Agent, which is detected and adjusted to 160mg/L, packing, is stored in -20 DEG C.Using preceding taking-up, and it is diluted to standard dilutions different dense Immunoglobulin E standard items (the immunoglobulin E antigen concentration of degree:0mg/L、20mg/L、40mg/L、70mg/L、100mg/ L).Then the membrane filtration with 0.45 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 5
Reagent R1:
MOPS buffer solutions 150mmol/L
Sodium chloride 30g/L
Sodium azide 1g/L
Macrogol 6000 55g/L
Nonidet P40 33g/L
Reagent R2:
MOPS buffer solutions 100mmol/L
Sodium chloride 30g/L
Sodium azide 1g/L
Goat anti-human immunoglobulin's E antibody 100mg/L
Nonidet P40 29g/L
Magnesium sulfate 7g/L
Calcium acetate 12g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (100mmol/L TRIS buffer solutions, 30g/L sodium chloride, 0.5g/L Sodium azide, 90g/L glucans, 100g/L trehaloses, 100g/L sucrose, 100g/L bovine serum albumin(BSA)s) dissolving, with commercially available control Reagent, which is detected and adjusted to 120mg/L, packing, is stored in -20 DEG C.Difference is diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (the immunoglobulin E antigen concentration of concentration:0mg/L、20mg/L、50mg/L、80mg/L、100mg/ L).Then the membrane filtration with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 6
Reagent R1:
Reagent R2:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Goat anti-human immunoglobulin's E antibody 10mg/L
Nonidet P40 0.9g/L
Magnesium sulfate 0.01g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (25mmol/L phosphate buffers, 2g/L sodium chloride, 0.2g/L Sodium azide, 0.3g/L glucans, 1g/L trehaloses, 3g/L sucrose, 3g/L bovine serum albumin(BSA)s) dissolving, with commercially available contrast agents Detect and adjust to 120mg/L, packing and be stored in -20 DEG C.Various concentrations are diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (immunoglobulin E antigen concentration:0mg/L、10mg/L、20mg/L、50mg/L、70mg/L).So Membrane filtration afterwards with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 7
Reagent R1:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Macrogol 6000 1g/L
Nonidet P40 0.9g/L
Reagent R2:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Goat anti-human immunoglobulin's E antibody 10mg/L
Nonidet P40 0.9g/L
Calcium acetate 0.01g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (20mmol/L phosphate buffers, 2g/L sodium chloride, 0.2g/L Sodium azide, 0.3g/L glucans, 1g/L trehaloses, 2g/L sucrose, 2g/L bovine serum albumin(BSA)s) dissolving, with commercially available contrast agents Detect and adjust to 120mg/L, packing and be stored in -20 DEG C.Various concentrations are diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (immunoglobulin E antigen concentration:0mg/L、10mg/L、20mg/L、50mg/L、70mg/L).So Membrane filtration afterwards with 0.65 μm is degerming, places 2~8 DEG C of preservations.
The immunoglobulin E detection kit of embodiment 8
Reagent R1:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Macrogol 6000 1g/L
Polysorbas20 0.9g/L
Reagent R2:
TRIS buffer solutions 20mmol/L
Sodium chloride 1g/L
Sodium azide 0.5g/L
Goat anti-human immunoglobulin's E antibody 10mg/L
Polysorbas20 0.9g/L
Calibration object:
Immunoglobulin E antigen standard dilutions (20mmol/L phosphate buffers, 2g/L sodium chloride, 0.2g/L Sodium azide, 0.3g/L glucans, 1g/L trehaloses, 2g/L sucrose, 2g/L bovine serum albumin(BSA)s) dissolving, with commercially available contrast agents Detect and adjust to 120mg/L, packing and be stored in -20 DEG C.Various concentrations are diluted to using preceding taking-up, and with standard dilutions Immunoglobulin E standard items (immunoglobulin E antigen concentration:0mg/L、10mg/L、20mg/L、50mg/L、70mg/L).So Membrane filtration afterwards with 0.65 μm is degerming, places 2~8 DEG C of preservations.
Different embodiment testing results compare, wherein CV values=STDEV (1-7)/average.
1. preparing the sample that a immunoglobulin E concentration is 40mg/L, sample is repeated to examine with the kit of embodiment 1 Survey 7 times, testing result is as shown in table 1.
Table 1:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 1, the immunoglobulin E concentration that embodiment 1 measured 1 month, 3 months, 12 months is close to true Value, and the coefficient of variation (CV values) measured is respectively less than 2%, illustrates that the kit of the present invention is reproducible, stable performance, measurement Accurately.
2. preparing the sample that a immunoglobulin E concentration is 1.0mg/L, sample is repeated with the kit of embodiment 2 Detection 7 times, testing result is as shown in table 2.
Table 2:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 2, the immunoglobulin E concentration that embodiment 2 measured 1 month, 3 months, 12 months is close to true Value, and the coefficient of variation measured is respectively less than 2%, illustrates that the kit of the present invention is reproducible, stable performance, measurement is accurate.
3. preparing the sample that a immunoglobulin E concentration is 25mg/L, sample is repeated to examine with the kit of embodiment 3 Survey 7 times, testing result is as shown in table 3.
Table 3:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 3, the immunoglobulin E concentration that embodiment 3 measured 1 month, 3 months, 12 months is close to true Value, and the coefficient of variation measured is respectively less than 1%, illustrates that the kit of the present invention is reproducible, stable performance, measurement is accurate.
4. preparing the sample that a immunoglobulin E concentration is 70mg/L, sample is repeated to examine with the kit of embodiment 4 Survey 7 times, testing result is as shown in table 4.
Table 4:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 4, the immunoglobulin E concentration that embodiment 4 measured 1 month, 3 months, 12 months is close to true Value, and the coefficient of variation measured is respectively less than 1%, illustrates that the kit of the present invention is reproducible, stable performance, measurement is accurate.
5. preparing the sample that a immunoglobulin E concentration is 25mg/L, sample is repeated to examine with the kit of embodiment 5 Survey 7 times, testing result is as shown in table 5.
Table 5:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 5, embodiment 5 is actual value in the immunoglobulin E concentration that 1 month, 3 months, 12 months measure, And the coefficient of variation measured is respectively less than 0.05%, illustrate that the kit of the present invention is reproducible, stable performance, measurement is accurate.
6. preparing the sample that a immunoglobulin E concentration is 40mg/L, sample is repeated to examine with the kit of embodiment 6 Survey 7 times, testing result is as shown in table 6.
Table 6:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 6, embodiment 6 deviates truly in the immunoglobulin E concentration that 1 month, 3 months, 12 months measure Value, and the coefficient of variation measured is all higher than 4%, illustrates that the kit repeatability is bad, performance is unstable, and measurement is inaccurate.
7. preparing the sample that a immunoglobulin E concentration is 40mg/L, sample is repeated to examine with the kit of embodiment 7 Survey 7 times, testing result is as shown in table 7.
Table 7:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 7, embodiment 7 deviates truly in the immunoglobulin E concentration that 1 month, 3 months, 12 months measure Value, and the coefficient of variation measured is all higher than 4%, illustrates that the kit repeatability is bad, performance is unstable, and measurement is inaccurate.
8. preparing the sample that a immunoglobulin E concentration is 40mg/L, sample is repeated to examine with the kit of embodiment 8 Survey 7 times, testing result is as shown in table 8.
Table 8:2-8 DEG C preserves 1 month, 3 months, 12 months measurement results
From table 8, embodiment 8 deviates truly in the immunoglobulin E concentration that 1 month, 3 months, 12 months measure Value, and the coefficient of variation measured is all higher than 5%, illustrates that the kit repeatability is bad, performance is unstable, and measurement is inaccurate.
It should be understood that the present invention disclosed is not limited only to specific method, scheme and the material of description, because these Equal alterable.It will also be understood that purpose of the terminology used here just for the sake of the specific embodiment scheme of description, rather than It is intended to limit the scope of the present invention, the scope of the present invention is limited solely by appended claim.
Those skilled in the art, which will also be appreciated that or be able to confirm that, uses no more than normal experiment, institute herein The many equivalents for the specific embodiment of the invention stated.These equivalents are also contained in appended claim.

Claims (10)

  1. A kind of 1. immunoglobulin E detection kit, it is characterised in that:The kit includes reagent R1 and reagent R2, described Included in reagent R1 in Nonidet P40 0.9-50g/L, the reagent R2 and include Nonidet P40 0.9- 50g/L, magnesium salts 0.01-15g/L, calcium acetate 0.01-20.5g/L and antibody 10-1000mg/L.
  2. 2. immunoglobulin E detection kit according to claim 1, it is characterised in that:Ethylo benzene in the reagent R1 Base polyethylene glycol is 4.5-42g/L, preferably 33g/L;Nonidet P40 is 5-42g/L in the reagent R2, preferably For 29g/L.
  3. 3. immunoglobulin E detection kit according to claim 1 or 2, it is characterised in that:The magnesium salts is 0.05- 10g/L, preferably 7g/L;The magnesium salts is preferably the one or more in magnesium sulfate, magnesium chloride or magnesium acetate.
  4. 4. according to the immunoglobulin E detection kit described in claim any one of 1-3, it is characterised in that:The calcium acetate For 0.05-15g/L, preferably 12g/L.
  5. 5. according to the immunoglobulin E detection kit described in claim any one of 1-4, it is characterised in that:The reagent R1 In also include buffer solution, inorganic salts, preservative and aggregation;Preferably, buffer solution 20- is also included in the reagent R1 150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L and aggregation 1-60g/L.
  6. 6. according to the immunoglobulin E detection kit described in claim any one of 1-5, it is characterised in that:The reagent R2 In also include buffer solution, inorganic salts and preservative, it is preferable that in the reagent R2 also comprising buffer solution 20-100mmol/L, nothing Machine salt 1-30g/L and preservative 0.5-1g/L.
  7. 7. according to the immunoglobulin E detection kit described in claim any one of 1-6, it is characterised in that:The kit Comprising calibration object, the calibration object is calibrated using multiple spot, and the calibration object includes buffer solution 20-100mmol/L, inorganic salts 1- 30g/L, preservative 0.1-2g/L, glucan 0.3-100g/L, trehalose 1-100g/L, sucrose 1-100g/L, bovine serum albumin White 1-100g/L and antigen.
  8. A kind of 8. immunoglobulin E detection kit, it is characterised in that:The kit includes reagent R1 and reagent R2, described Buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, Macrogol 6000 1- are included in reagent R1 60g/L, Nonidet P40 0.9-50g/L;Buffer solution 20-100mmol/L, inorganic salts 1- are included in the reagent R2 30g/L, preservative 0.5-1g/L, antibody 10-1000mg/L, Nonidet P40 0.9-50g/L, magnesium sulfate 0.01- 15g/L, calcium acetate 0.01-20.5g/L;
    Preferably,
    Buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, polyethylene glycol are included in the reagent R1 6000 1-60g/L, Nonidet P40 4.5-42g/L;Buffer solution 20-100mmol/L, nothing are included in the reagent R2 Machine salt 1-30g/L, preservative 0.5-1g/L, antibody 10-1000mg/L, Nonidet P40 5-42g/L, magnesium sulfate 0.05-10g/L, calcium acetate 0.05-15g/L;
    It is highly preferred that
    Buffer solution 20-150mmol/L, inorganic salts 1-30g/L, preservative 0.5-1g/L, polyethylene glycol are included in the reagent R1 6000 1-60g/L, Nonidet P40 33g/L;Buffer solution 20-100mmol/L, inorganic salts are included in the reagent R2 1-30g/L, preservative 0.5-1g/L, antibody 10-1000mg/L, Nonidet P40 29g/L, magnesium sulfate 7g/L, acetic acid Calcium 12g/L.
  9. 9. according to the immunoglobulin E detection kit described in claim any one of 1-8, it is characterised in that:
    The antibody is preferably goat-anti people, rabbit-anti people, horse is anti-human, mouse is anti-human or other animal anti-human antibodies;
    The buffer solution is preferably that acetate buffer, ammonium chloride buffer, phosphate buffer, TRIS buffer solutions, boric acid delay One or more in fliud flushing, glycine buffer, CAPSO, MOPS or Hepes buffer solution;
    The inorganic salts are preferably one or both of sodium chloride, potassium chloride;
    The preservative is preferably Sodium azide, phenol, P-hydroxybenzoic acid, ethyl-para-hydroxybenzoate or ethyl mercury thiosulfuric acid One or more in sodium;
    The aggregation is preferably in polyethylene glycol 2000, Macrogol 4000, Macrogol 6000 or PEG 8000 It is one or more of.
  10. 10. a kind of detection method using above-mentioned immunoglobulin E detection kit, comprise the following steps:
    (1) add reagent R1 into testing sample to mix, testing sample and reagent R1 are (1-9) by volume:300 add, and 37 DEG C be incubated, under certain wavelength, read absorbance A 1;
    (2) add reagent R2 into the mixed liquor of step (1) to mix, reagent R2 and reagent R1 is 1 by volume:(1-6) is added, 37 DEG C of incubations, under certain wavelength, read absorbance A 2;
    (3) absorbance △ A, △ A=A2-A1 are drawn;
    (4) use calibration object on automatic clinical chemistry analyzer by built-in curve matching model fitting standard curve, according to suction Luminosity calculates the content of immunoglobulin E in testing sample automatically.
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Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102798725A (en) * 2012-08-13 2012-11-28 沃克(天津)生物科技有限公司 Diagnostic kit for determination of serum total IgE, preparation method and application method
CN105137062A (en) * 2015-06-03 2015-12-09 章丘维他力医疗器械有限公司 Immunoglobulin E immunoturbidimetry detection kit
CN105717300A (en) * 2016-02-02 2016-06-29 潍坊三维生物工程集团有限公司 Kit and method for detecting content of immune globulin E and application of kit
JP2016200430A (en) * 2015-04-08 2016-12-01 株式会社パートナーファーム Tear collection and inspection tool
US20170089893A1 (en) * 2015-09-24 2017-03-30 Globallergy, Llc Chromatographic immune assay for the detection of allergic sensitivities

Patent Citations (5)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN102798725A (en) * 2012-08-13 2012-11-28 沃克(天津)生物科技有限公司 Diagnostic kit for determination of serum total IgE, preparation method and application method
JP2016200430A (en) * 2015-04-08 2016-12-01 株式会社パートナーファーム Tear collection and inspection tool
CN105137062A (en) * 2015-06-03 2015-12-09 章丘维他力医疗器械有限公司 Immunoglobulin E immunoturbidimetry detection kit
US20170089893A1 (en) * 2015-09-24 2017-03-30 Globallergy, Llc Chromatographic immune assay for the detection of allergic sensitivities
CN105717300A (en) * 2016-02-02 2016-06-29 潍坊三维生物工程集团有限公司 Kit and method for detecting content of immune globulin E and application of kit

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