CN108776232A - A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit and preparation method thereof - Google Patents

A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit and preparation method thereof Download PDF

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CN108776232A
CN108776232A CN201810941310.1A CN201810941310A CN108776232A CN 108776232 A CN108776232 A CN 108776232A CN 201810941310 A CN201810941310 A CN 201810941310A CN 108776232 A CN108776232 A CN 108776232A
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antibody
hgh
growth hormone
human growth
biotin
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翟涛
刘杨
何浩会
高威
孙成艳
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Dirui Medical Technology Co Ltd
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Dirui Medical Technology Co Ltd
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    • 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
    • G01N33/74Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving hormones or other non-cytokine intercellular protein regulatory factors such as growth factors, including receptors to hormones and growth factors

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Abstract

A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit of present invention offer and preparation method thereof, belongs to technical field of immunoassay.The kit includes:Be coated with the bead suspension of Streptavidin, the GH antibody of acridinium ester label and biotin labeling GH antibody.The present invention also provides a kind of preparation methods of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit.The kit is using the GH in sandwich method principle quantitative determination serum or blood plasma, biotin-GH antibody complexes are added in Streptavidin-magnetic particle suspension, pass through the compatible reaction of biotin and Streptavidin, form magnetic microsphere-Avidin-Biotin-GH compounds, pass through antigen-antibody reaction, it forms antigen antibody complex and forms magnetic particle-biotin-GH antibody-GH-GH antibody-acridinium ester, the detection method has the advantages that high sensitivity, high specificity, reproducible, detection range is wide, advantage of lower cost, can be widely used for clinical detection.

Description

A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit and its preparation Method
Technical field
The invention belongs to technical field of immunoassay, are related to a kind of detection human growth hormone (HGH) chemiluminscence immunoassay Kit and preparation method thereof.
Background technology
Human growth hormone (HGH) (human Growth Hormone) is the single peptide secreted by anteriorpituitary acidophic cell Chain protein hormone is made of 191 amino acid, and there is extensive physiological function, the growth hormone of the mankind mainly to pass through stimulation Hepatic secretion insulin-like growth factor (IGF-I), acts on bone and cartilage, causes the growth of height, while can promote people Body protein matter synthesizes and lipolysis, adjusts internal water salt balance.
1. the clinical manifestation of auxin exception
Growth hormone is broadly divided into extremely:1) growth hormone is excessive;2) growth hormone deficiency.Growth hormone excessively would generally There is gigantism and acromegalia.Gigantism is a kind of abnormal longitudinal growth, the reason is that hGH and IGF-1 over effects, add Upper epiphyseal growth plate childhood open cause stature excessively high.Acromegalia is also a kind of disease caused by hGH and IGF-1 excess Disease occurs after manhood growth plate cartilage fusion.The diverse clinical manifestations of acromegalia, existing slight sign, such as Acra hyperplasia and facial characteristics roughening, apparent metabolism, angiocarpy and the respiratory tract for also thering are morbidity and mortality to be risen The form of expression.Children growth anhormonia can make longitudinal growth more slow compared to the stone age, and if being grown up has serious growth to swash Element, which lacks, will appear muscular strength decline, and bone amount is reduced, and insulin sensitivity declines, and abdominal obesity and cardiovascular risk factors increase (i.e. dyslipidemia is horizontal, atherosclerosis).Kidney, bone and the intestinal cell pair of the adult of progressive growth anhormonia Parathormone (PTH) is insensitive, and then generates slight PTH and resist, and with the raising of serum PTH levels.With end-organ Official's sensitivity decline is consistent, is similarly postponed to the blood calcium reaction of PTH.
2. the detection method of growth hormone
The method of currently used detection growth hormone has radioimmunoassay technique (RIA), ELISA technology (ELISA), but both methods there are many deficiencies, such as RIA there are radioactive pollution, marker half-life short, to operator Have the shortcomings that radioactive damage, cumbersome, detection time is long;ELISA have sensitivity is low, detection range is narrow, detection when Between long, poor repeatability the shortcomings of.
Invention content
The purpose of the present invention is to solve it is existing detection growth hormone method detection time it is long, sensitivity is low, again The problem of renaturation difference, and a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit is provided and preparation method thereof.
Present invention firstly provides a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit, the kit packets It includes:
It is coated with the bead suspension of Streptavidin
The GH antibody of acridinium ester label
The GH antibody of biotin labeling
Preferably, described to be coated in the bead suspension of Streptavidin, it is coated with the magnetic bead of Streptavidin Grain size be 1-3 μm.
Preferably, in the GH antibody of the acridinium ester label, the molar ratio of acridinium ester and GH antibody is (3-15):1.
Preferably, in the GH antibody of the biotin labeling, the molar ratio of biotin and GH antibody is (3-15):1.
Preferably, the kit further includes calibration object and quality-control product.
The invention also includes a kind of preparation method of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit, packets It includes:
Step 1:It is coated with the preparation of the bead suspension of Streptavidin
After Streptavidin magnetic particle solution and TBST solution mixings, be placed on magnetic separator, until supernatant without Muddiness abandons supernatant, leaves and takes magnetic particle, is made into solid-phase reagent R1 after cleaning in buffer solution;
Step 2:The preparation of the GH antibody of acridinium ester label
GH antibody is put into centrifuge tube and is centrifuged, carbonic acid buffer is then added, the centrifugation of acridine ester solution is added after mixing, It is protected from light being put into after the centrifugation seal of tube in magazine, magazine is then put into mixing in gas bath constant temperature oscillator, confining liquid is added, puts Enter mixing in gas bath constant temperature oscillator, by the antibody closed by purifying, collection, be then placed in buffer solution and dilute, preserve, Obtain R2 reagents;
Step 3:The preparation of the GH antibody of biotin labeling
GH antibody is taken, ultrafiltration centrifugation is carried out, GH antibodies buffers is replaced into PBS, it is abundant that biotin solution is then added The biotin labelled antibodies being collected into after being placed at room temperature for 2-4 hours, are selected buffer solution dilution, obtain R3 reagents by mixing;
Preferably, the buffer solution of the step 1 be 50mM MES, 0.05% tween, 0.05%Proclin300, pH6.0。
Preferably, in the step 2 GH antibody quality (μ g):The volume (μ l) of acridine ester solution is 100:1.
Preferably, the confining liquid of the step 2 is preferably lysine, mass fraction 20%.
Preferably, the step 2 buffer solution be 50mM MES, 0.05% Tween-20,0.05%Proclin300, pH6.0。
Preferably, the buffer solution of the step three is to contain 1%BSA, the 100mM citrate buffer solutions that PH is 6.0.
Beneficial effects of the present invention
A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit of present invention offer and preparation method thereof, should Kit is added using the GH in sandwich method principle quantitative determination serum or blood plasma in Streptavidin-magnetic particle suspension Biotin-GH antibody complexes form magnetic microsphere-Avidin-biology by the compatible reaction of biotin and Streptavidin Element-GH compounds form antigen antibody complex and form magnetic particle-biotin-GH antibody-GH-GH by antigen-antibody reaction Compound is adsorbed on reaction cup bottom by antibody-acridinium ester with magnetic field, washes off free ingredient, and soda acid exciting liquid is added, according to The content of GH in luminous intensity quantitative measurment sample.The present invention combines chemiluminescence and Enzyme Immunoassay, The detection method has the advantages that high sensitivity, high specificity, reproducible, detection range is wide, advantage of lower cost, can be extensive For clinical detection.
Description of the drawings
Fig. 1 is the preparation flow design of the preparation method of the present inventor's growth hormone chemiluminescence immune detection reagent kit Figure.
Fig. 2 is to survey relative light unit using the detection calibration product examine of the present inventor's growth hormone chemiluminescence quantification kit Standard curve.
Specific implementation mode
Present invention firstly provides a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit, the kit packets It includes:
It is coated with the bead suspension of Streptavidin
The GH antibody of acridinium ester label
The GH antibody of biotin labeling
According to the present invention, described is coated in the bead suspension of Streptavidin, is coated with the magnetic of Streptavidin The grain size of pearl is preferably 1-3 μm, when being coated with the grain size of magnetic bead of Streptavidin less than 1 μm, antigen or antibody and magnetic Pearl Percentage bound is low, and whole light quantity subnumber may be caused relatively low;When being coated with the grain size of magnetic bead of Streptavidin higher than 3 μm, Non-specific binding is with obvious effects, may lead to kit poor sensitivity etc..
According to the present invention, in the GH antibody of the acridinium ester label, the molar ratio of acridinium ester and GH antibody is preferably (3- 15):1.
According to the present invention, in the GH antibody of the biotin labeling, the molar ratio of biotin and GH antibody is preferred (3- 15):1.
According to the present invention, the kit further includes calibration object and quality-control product.The system of the calibration object and quality-control product It is standby identical, it preferably includes:
GH is diluted to calibration object with the 100mM PBS buffer solution containing 20% calf serum, be distributed into 0.03ng/ml, 0.1ng/ml、0.5ng/ml、1ng/ml、2ng/ml、5ng/ml、10ng/ml、25ng/ml、50ng/ml。
The invention also includes a kind of preparation method of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit, tools Body flow is as shown in Figure 1, include:
Step 1:It is coated with the preparation of the bead suspension of Streptavidin
After Streptavidin magnetic particle solution and TBST solution mixings, be placed on magnetic separator, until supernatant without Muddiness abandons supernatant, leaves and takes magnetic particle, is made into solid-phase reagent R1 after cleaning in buffer solution;The Streptavidin magnetic particle The concentration of solution is preferably 100mg/ml;Streptavidin magnetic particle solution and the volume ratio of TBST solution are preferably 0.5:10; Buffer solution is 50mM MES, 0.05% tween, 0.05%Proclin300, pH6.0;The solid-phase reagent coating strepto- is affine The magnetic bead concentration of element is preferably 0.05%-0.1%;
Step 2:The preparation of the GH antibody of acridinium ester label
GH antibody is put into centrifuge tube and is centrifuged, preferably centrifuges 10s~30s at room temperature, ensures that antibody is located at centrifuge tube Then bottom position is added carbonic acid buffer, the centrifugation of acridine ester solution is added after mixing, the centrifuging temperature is preferably room Temperature, centrifugation time are preferably 0.5min~3min;It is protected from light being put into after the centrifugation seal of tube in magazine, magazine is then put into gas bath Mixing in constant temperature oscillator (25 DEG C), the mixing time is preferably 2-4h, and confining liquid is added, is put into gas bath constant temperature oscillator The closing of middle mixing, the off-period is preferably 1-2h, by 250 column purification of sephadex G on the antibody closed, uses PB Buffer solution elutes, and collects, is then placed in buffer solution and dilutes, and preserves, obtains R2 reagents;
The quality (μ g) of the GH antibody:The volume (μ l) of acridine ester solution is preferably 100:1;The change acridinium ester The concentration of solution is preferably 2mg/mL;The confining liquid is preferably lysine, and mass fraction is preferably 20%;The buffering Liquid is 50mM MES, 0.05% Tween-20,0.05%Proclin300, pH6.0;The GH of the R2 reagent acridinium ester labels Antibody concentration is preferably 1-3ug/mL;
Step 3:The preparation of the GH antibody of biotin labeling
GH monoclonal antibodies are added in 50KDa ultra-filtration centrifuge tubes, PBS buffer solution is added, centrifugation is repeated 3 times, by antibody Interior buffer exchange is biotin labeling buffer solution, collects solution after displacement, in molar ratio antibody:Biotin is 1:3-1:15 add Enter biotin, stands 2-4h.The full-automatic protein purification instrument of GE company AKTA is selected to purify biotin labelled antibodies solution, Purified solution is collected, purified antibodies are formulated as R3 reagents, 4 DEG C of preservations with containing citrate buffer solution;
The quality (μ g) of the GH monoclonal antibodies:The volume (μ l) of PBS buffer solution is preferably 3:1;The PBS is slow The concentration of fliud flushing is preferably 50mM-200mM;The centrifugal rotational speed is preferably 8000-12000rpm, and centrifugation time is preferably 5- 15min;The GH antibody concentrations of the R3 reagent biotin labelings are preferably 1-3ug/mL;The citrate buffer solution be containing There are 1%BSA, the 100mM citrate buffer solutions that PH is 6.0.
The detecting step of kit of the present invention:Sample to be tested and R2 reagents are incubated 5min, R3 and R1 reagents are added and are incubated Exciting liquid record relative luminous intensity (RLU) is added in 5min, washing.In a certain range, the content and relative luminous intensity of GH It is directly proportional.
The kit of the present invention is using the GH in sandwich method principle quantitative determination serum or blood plasma, in Streptavidin-magnetic Biotin-GH antibody complexes are added in microparticle suspending liquid, by the compatible reaction of biotin and Streptavidin, it is micro- to form magnetic Ball-Avidin-Biotin-GH compounds forms antigen antibody complex and forms magnetic particle-biology by antigen-antibody reaction Element-GH antibody-GH-GH antibody-acridinium ester washes off free ingredient by magnetic separator separating immune complexes.Pass through soda acid Exciting liquid excites acridinium ester to shine, record relative luminous intensity (RLU), in the range of linearity, in sample the content of GH with it is opposite Luminous intensity is directly proportional.
Further detailed description is done to the present invention with reference to specific embodiment.
Embodiment 1 prepares the GH chemiluminescence detection kits of the present invention
One, the preparation of calibration object
GH is diluted to calibration object with the 100mM PBS buffer solution containing 20% calf serum, be distributed into 0.03ng/ml, 0.1ng/ml、0.5ng/ml、1ng/ml、2ng/ml、5ng/ml、10ng/ml、25ng/ml、50ng/ml。
Two, the R1 solution of coating Streptavidin MagneSphere is prepared
The Streptavidin magnetic particle solution 0.5 milliliter (50mg) of a concentration of 100mg/ml is taken, 10 milliliters of TBST is added Solution mixes well after ten minutes, is positioned on magnetic separator, until supernatant without muddiness, abandons supernatant, leaves and takes magnetic particle.It repeats clear It is a concentration of in 50mM MES, 0.05% tween, 0.05%Proclin300, the buffer solution of pH6.0 it to be made into magnetic bead after washing 3 times 0.05% solid-phase reagent, 2~8 DEG C of preservations.
Three, the preparation of the GH monoclonal antibody R2 solution of acridinium ester label
500ug antibody is put into centrifuge tube, ensures that antibody is located at centrifuge tube bottom position (centrifuge room temperature centrifuges 20s) After carbonate buffer solution is added, mix well, the DMF solution of 5 μ l 2mg/mL acridinium esters be added after mixing, with centrifuge room temperature Under the conditions of centrifuge 0.5 minute.It will centrifuge to be put into after effective sealed membrane seals and be protected from light in magazine, magazine is put into gas bath constant temperature later Oscillator (25 DEG C), mixing 4 hours.20% lysine confining liquids of 1mL are added, are put into gas bath constant temperature oscillator (25 DEG C), middling speed Mixing, off-period 1h.It by 250 column purification of sephadex G on the antibody closed, is eluted with PB buffer solutions, branch receives Collection.The antibody-solutions gathered are positioned over 2~8 DEG C of preservations.When use by after purification GH antibody concentrated solutions 50mM MES, The buffer solution of 0.05% tween, 0.05%Proclin300, pH6.0 are diluted to final concentration of 0.1ug/ml, 2~8 DEG C of preservations.
Four, the preparation of the GH monoclonal antibody R3 solution of biotin labeling
GH monoclonal antibodies 300ug is added in 50KDa ultra-filtration centrifuge tubes, the 100mMPBS buffer solutions of 500ul are added, 10000rpm centrifuges 10min, is repeated 3 times, and is biotin labeling buffer solution by buffer exchange in antibody.It collects molten after replacing Liquid, by antibody:Biotin=1:Biotin is added in 15 molar ratios, stands 2h.Select the full-automatic protein purification instrument of GE company AKTA Biotin labelled antibodies solution is purified, purified solution is collected, with containing 1%BSA, the 100mM citric acids that PH is 6.0 Purified antibodies are formulated as the R3 solution of 0.5ug/ml, 4 DEG C of preservations by buffer solution.
Embodiment 2 prepares the GH chemiluminescence detection kits of the present invention
One, the preparation of calibration object
GH is diluted to calibration object with the 100mM PBS buffer solution containing 20% calf serum, be distributed into 0.03ng/ml, 0.1ng/ml、0.5ng/ml、1ng/ml、2ng/ml、5ng/ml、10ng/ml、25ng/ml、50ng/ml。
Two, the R1 solution of coating Streptavidin MagneSphere is prepared
The Streptavidin magnetic particle solution 0.5 milliliter (50mg) of a concentration of 100mg/ml is taken, 10 milliliters of TBST is added Solution mixes well after ten minutes, is positioned on magnetic separator, until supernatant without muddiness, abandons supernatant, leaves and takes magnetic particle.It repeats clear It is a concentration of in 50mM MES, 0.05% tween, 0.05%Proclin300, the buffer solution of pH6.0 it to be made into magnetic bead after washing 3 times 0.03% solid-phase reagent, 2~8 DEG C of preservations.
Three, the preparation of the GH monoclonal antibody R2 solution of acridinium ester label
500ug antibody is put into centrifuge tube, ensures that antibody is located at centrifuge tube bottom position (centrifuge room temperature centrifuges 20s) After carbonate buffer solution is added, mix well, the DMF solution of 5 μ l 2mg/mL acridinium esters be added after mixing, with centrifuge room temperature Under the conditions of centrifuge 10s.It will centrifuge to be put into after effective sealed membrane seals and be protected from light in magazine, magazine is put into gas bath constant temperature oscillation later Device (37 DEG C), mixing 3 hours.20% lysine confining liquids of 1mL are added, are put into gas bath constant temperature oscillator (37 DEG C), middling speed is mixed It is even, off-period 45min.It by 250 column purification of sephadex G on the antibody closed, is eluted with PB buffer solutions, branch receives Collection.The antibody-solutions gathered are positioned over 2~8 DEG C of preservations.When use by after purification GH antibody concentrated solutions 50mM MES, The buffer solution of 0.05% tween, 0.05%Proclin300, pH6.0 are diluted to final concentration of 0.05ug/ml, 2~8 DEG C of preservations.
Four, the preparation of the GH monoclonal antibody R3 solution of biotin labeling
GH monoclonal antibodies 300ug is added in 50KDa ultra-filtration centrifuge tubes, the 100mM PBS buffer solution of 500ul is added, 12000rpm centrifuges 8min, is repeated 3 times, and is biotin labeling buffer solution by buffer exchange in antibody.Solution after replacing is collected, By antibody:Biotin=1:Biotin is added in 10 molar ratios, stands 3h.Select the full-automatic protein purification instrument of GE company AKTA to life Object element labelled antibody solution is purified, and purified solution is collected, with containing 1%BSA, the 100mM lemon acid bufferings that PH is 6.0 Purified antibodies are formulated as the R3 solution of 1ug/ml, 4 DEG C of preservations by liquid.
Embodiment 3 prepares the GH chemiluminescence detection kits of the present invention
One, the preparation of calibration object
GH is diluted to calibration object with the 100mM PBS buffer solution containing 20% calf serum, be distributed into 0.03ng/ml, 0.1ng/ml、0.5ng/ml、1ng/ml、2ng/ml、5ng/ml、10ng/ml、25ng/ml、50ng/ml。
Two, the R1 solution of coating Streptavidin MagneSphere is prepared
The Streptavidin magnetic particle solution 0.5 milliliter (50mg) of a concentration of 100mg/ml is taken, 10 milliliters of TBST is added Solution mixes well after ten minutes, is positioned on magnetic separator, until supernatant without muddiness, abandons supernatant, leaves and takes magnetic particle.It repeats clear It is a concentration of in 50mM MES, 0.05% tween, 0.05%Proclin300, the buffer solution of pH6.0 it to be made into magnetic bead after washing 3 times 0.03% solid-phase reagent, 2~8 DEG C of preservations.
Three, the preparation of the GH monoclonal antibody R2 solution of acridinium ester label
500ug antibody is put into centrifuge tube, ensures that antibody is located at centrifuge tube bottom position (centrifuge room temperature centrifuges 20s) After carbonate buffer solution is added, mix well, the DMF solution of 5 μ l 2mg/mL acridinium esters be added after mixing, with centrifuge room temperature Under the conditions of centrifuge 30s.It will centrifuge to be put into after effective sealed membrane seals and be protected from light in magazine, magazine is put into gas bath constant temperature oscillation later Device (37 DEG C), mixing 2 hours.20% lysine confining liquids of 1mL are added, are put into gas bath constant temperature oscillator (37 DEG C), middling speed is mixed It is even, off-period 30min.It by 250 column purification of sephadex G on the antibody closed, is eluted with PB buffer solutions, branch receives Collection.The antibody-solutions gathered are positioned over 2~8 DEG C of preservations.When use by after purification GH antibody concentrated solutions 50mM MES, The buffer solution of 0.05% tween, 0.05%Proclin300, pH6.0 are diluted to final concentration of 0.07ug/ml, 2~8 DEG C of preservations.
Four, the preparation of the GH monoclonal antibody R3 solution of biotin labeling
GH monoclonal antibodies 300ug is added in 50KDa ultra-filtration centrifuge tubes, the 100mM PBS buffer solution of 500ul is added, 9000rpm centrifuges 10min, is repeated 3 times, and is biotin labeling buffer solution by buffer exchange in antibody.Solution after replacing is collected, By antibody:Biotin=1:Biotin is added in 3 molar ratios, stands 4h.Select the full-automatic protein purification instrument of GE company AKTA to life Object element labelled antibody solution is purified, and purified solution is collected, with containing 1%BSA, the 100mM lemon acid bufferings that PH is 6.0 Purified antibodies are formulated as the R3 solution of 1.5ug/ml, 4 DEG C of preservations by liquid.
Embodiment 4GH chemical luminous immune detection methods
With Full-automatic chemiluminescence immunoassay analysis meter (CM-180) for detection instrument, methodology pattern is double-antibody sandwich Method, i.e. instrument sequentially add the sample of 20 μ l, the GH monoclonal antibodies of biotin labeling of 50 μ l, 50 μ l chemiluminescent substance The GH monoclonal antibodies of label after reacting 10min, then add 40 μ l Streptavidin magnetic particles, after reacting 10min, carry out magnetic point From addition cleaning solution cleans 5 times, and instrument will react compound and be sent into detector, sequentially add preexciting liquid and exciting liquid progress Luminescence-producing reaction acquires optical signal, records luminous value.
Embodiment 5GH chemiluminescence immune detection reagent kit performance evaluations
GH chemiluminescence detection kits obtained are examined and determine according to professional standard in this field and vertification regulation, are tied Fruit is as follows:
1. the kit range of linearity measures
By the kit of preparation wherein 1 batch, measure range of linearity sample 0.03ng/ml, 0.1ng/ml, 0.5ng/ml, 1ng/ml, 2ng/ml, 5ng/ml, 10ng/ml, 25ng/ml, 50ng/ml show that the range of linearity is 0.03ng/mL~50ng/ ML, linearly dependent coefficient r >=0.9900.Fig. 2 is the test school using the present inventor's growth hormone chemiluminescence quantification kit The standard curve of relative light unit is surveyed in quasi- product examine, and abscissa is concentration, and unit ng/ml, ordinate is luminous value.As a result such as table Shown in 1:
1 calibration object concentration of table and relative luminous intensity
2. the measurement of kit sensitivity
By the kit of preparation wherein 1 batch, 20 zero-dose samples are measured, average value (M) and standard deviation (SD) is calculated, obtains Go out M+2SD, carrying out 2 regression fits according to the concentration-RLU between zero-dose calibration object and adjacent calibration object obtains first power Journey brings the RLU of M+2SD into equations, show that respective concentration value is kit sensitivity 0.0011ng/ml.1st luminous value The results are shown in Table 2:
2 blank sample luminous value of table
First point of mean value M that shines1=52.65, SD1=19.58, M1+2SD1=91.80
2nd luminous value is as shown in table 3:
3 second point of table calibrates luminous value
The luminous mean value M=7302 of second point
First point (0,52.65) and second point (0.2,7302) line matched curve, sensitivity=0.0011ng/ of calculating ml。
3. kit precision is tested
(1) withinrun precision
By the kit of preparation wherein 1 batch, replication is distinguished 10 times to the sample of two various concentrations of high level and low value, Show that variation within batch coefficient is 1.66%-3.61%.
4 kit withinrun precision of table measures
(2) betweenrun precision
By the kit of preparation wherein 1 batch, replication is distinguished 10 times to the sample of two various concentrations of high level and low value, Show that interassay coefficient of variation is 1.66%-3.61%.
5 kit betweenrun precision of table measures
4. kit accuracy determination
By the kit of preparation wherein 1 batch, measured concentration is the standard substance of 0.5ng/ml and 20ng/ml, relative deviation < 10%, test result is as follows:
6 kit accuracy determination of table
5. kit specificity experiments
GH detectable concentrations find following cross reaction when being 1ng/mL and 10ng/mL:
Table 7 kit specificity
6. stabilization of kit is tested
The kit of preparation is carried out to 4 DEG C and 37 DEG C of 14 days stability experiments respectively, the results showed that kit standard product are sent out The indexs such as variation, precision, the accuracy of luminous intensity are in normal range (NR), and the kit term of validity was up to 24 months.
By a large amount of repeated experiments, kit index of the invention is as follows:
Detection range:0.02-50ng/ml;
Sensitivity:Minimum detection limit is not higher than 0.0011ng/ml;
Precision:Less than 10%;
Accuracy:Measured value standard substance deviation is less than 10%.
Specificity:Measured concentration is not less than the prolactin(PRL sample of 2000mIU/L, and measurement result should be not more than 0.5ng/ ml。

Claims (10)

1. a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit, which is characterized in that the kit includes:
It is coated with the bead suspension of Streptavidin
The GH antibody of acridinium ester label
The GH antibody of biotin labeling.
2. a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1, feature It is, described is coated in the bead suspension of Streptavidin, and the grain size for being coated with the magnetic bead of Streptavidin is 1-3 μ m。
3. a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1, feature It is, in the GH antibody of the acridinium ester label, the molar ratio of acridinium ester and GH antibody is (3-15):1.
4. a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1, feature It is, in the GH antibody of the biotin labeling, the molar ratio of biotin and GH antibody is (3-15):1.
5. a kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1, feature It is, the kit further includes calibration object and quality-control product.
6. a kind of preparation side of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1 Method, which is characterized in that including:
Step 1:It is coated with the preparation of the bead suspension of Streptavidin
After Streptavidin magnetic particle solution and TBST solution mixings, it is placed on magnetic separator, until supernatant is without muddiness, Supernatant is abandoned, magnetic particle is left and taken, is made into solid-phase reagent R1 after cleaning in buffer solution;
Step 2:The preparation of the GH antibody of acridinium ester label
GH antibody is put into centrifuge tube and is centrifuged, is then added carbonic acid buffer, the centrifugation of acridine ester solution is added after mixing, it will be from It is put into and is protected from light in magazine after the heart seal of tube, magazine is then put into mixing in gas bath constant temperature oscillator, confining liquid is added, is put into gas Mixing in constant temperature oscillator is bathed, by the antibody closed by purifying, collection, is then placed in buffer solution and dilutes, preserve, obtain R2 reagents;
Step 3:The preparation of the GH antibody of biotin labeling
GH antibody is taken, ultrafiltration centrifugation is carried out, GH antibodies buffers is replaced into PBS, biotin solution is then added and mixes well, After being placed at room temperature for 2-4 hours, the biotin labelled antibodies being collected into are selected into buffer solution dilution, obtain R3 reagents.
7. a kind of preparation side of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 6 Method, which is characterized in that the buffer solution of the step 1 is 50mM MES, 0.05% tween, 0.05%Proclin300, pH6.0.
8. a kind of preparation side of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 6 Method, which is characterized in that the quality (μ g) of GH antibody in the step 2:The volume (μ l) of acridine ester solution is 100:1.
9. a kind of preparation side of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 6 Method, which is characterized in that the confining liquid of the step 2 is preferably lysine, mass fraction 20%.
10. a kind of preparation of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit according to claim 1 Method, which is characterized in that the step 2 buffer solution be 50mM MES, 0.05% Tween-20,0.05%Proclin300, pH6.0。
CN201810941310.1A 2018-08-17 2018-08-17 A kind of detection human growth hormone (HGH) chemical luminescence immune assay determination reagent kit and preparation method thereof Pending CN108776232A (en)

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CN110240644A (en) * 2019-06-28 2019-09-17 深圳市亚辉龙生物科技股份有限公司 Growth hormone receptor mutant, human growth hormone (HGH) immunogene, polyclonal antibody and detection kit
CN110308287A (en) * 2019-07-31 2019-10-08 宁波奥丞生物科技有限公司 A kind of preparation method of the chemical luminescence reagent kit of placenta growth factor
CN110579609A (en) * 2019-07-06 2019-12-17 湖南莱拓福生物科技有限公司 AKR1B10 chemiluminescence quantitative detection kit and application thereof
CN110779912A (en) * 2019-11-22 2020-02-11 无锡壹闪生物科技有限公司 Microsphere-free homogeneous chemiluminescence system of biotin-avidin or streptavidin
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CN113125740A (en) * 2021-05-17 2021-07-16 郑州安图生物工程股份有限公司 Method for identifying magnetic particle activation efficiency in chemiluminescence immunoassay technology
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CN109470872B (en) * 2018-12-07 2022-02-08 迈克生物股份有限公司 Magnetic particle buffer
CN110240644B (en) * 2019-06-28 2021-03-16 深圳市亚辉龙生物科技股份有限公司 Human growth hormone receptor mutant, human growth hormone immunogen, polyclonal antibody and detection kit
CN110240644A (en) * 2019-06-28 2019-09-17 深圳市亚辉龙生物科技股份有限公司 Growth hormone receptor mutant, human growth hormone (HGH) immunogene, polyclonal antibody and detection kit
CN110579609A (en) * 2019-07-06 2019-12-17 湖南莱拓福生物科技有限公司 AKR1B10 chemiluminescence quantitative detection kit and application thereof
CN110308287A (en) * 2019-07-31 2019-10-08 宁波奥丞生物科技有限公司 A kind of preparation method of the chemical luminescence reagent kit of placenta growth factor
CN110779912A (en) * 2019-11-22 2020-02-11 无锡壹闪生物科技有限公司 Microsphere-free homogeneous chemiluminescence system of biotin-avidin or streptavidin
CN110779912B (en) * 2019-11-22 2022-05-17 无锡壹闪生物科技有限公司 Biotin-avidin or streptavidin microsphere-free homogeneous chemiluminescence system
CN112362643A (en) * 2020-11-09 2021-02-12 长春金赛药业有限责任公司 Long-acting growth hormone immune quantitative detection kit based on lanthanide chemiluminescence method and method thereof
CN112816713A (en) * 2020-12-30 2021-05-18 北京联众泰克科技有限公司 Composition for human growth hormone detection, application of composition, magnetic microsphere electrochemiluminescence immunoassay kit and detection method
CN113125740A (en) * 2021-05-17 2021-07-16 郑州安图生物工程股份有限公司 Method for identifying magnetic particle activation efficiency in chemiluminescence immunoassay technology
CN113125740B (en) * 2021-05-17 2022-03-01 郑州安图生物工程股份有限公司 Method for identifying magnetic particle activation efficiency in chemiluminescence immunoassay technology
CN114778817A (en) * 2022-06-17 2022-07-22 山东中鸿特检生物科技有限公司 Kit for detecting interferon in serum and plasma, detection method and application
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Application publication date: 20181109