CN102659942B - Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit - Google Patents
Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit Download PDFInfo
- Publication number
- CN102659942B CN102659942B CN 201210160274 CN201210160274A CN102659942B CN 102659942 B CN102659942 B CN 102659942B CN 201210160274 CN201210160274 CN 201210160274 CN 201210160274 A CN201210160274 A CN 201210160274A CN 102659942 B CN102659942 B CN 102659942B
- Authority
- CN
- China
- Prior art keywords
- flagellin
- vibrio parahemolyticus
- monoclonal antibody
- enzyme
- test kit
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired - Fee Related
Links
Images
Landscapes
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
Abstract
The invention discloses a vibrio parahaemolyticus flagellin monoclonal antibody and an antigen capture ELISA (enzyme-linked immunosorbent assay) kit. The vibrio parahaemolyticus flagellin monoclonal antibody is produced by secreting of a hybridoma cell strain with the preservation number of CGMCC (China General Microbiological Culture Collection) No.6061. The vibrio parahaemolyticus flagellin monoclonal antibody can be used for detecting vibrio parahaemolyticus. The invention also discloses a vibrio parahaemolyticus flagellin capture ELISA (enzyme-linked immunosorbent assay) kit.
Description
Technical field
The invention belongs to field of immunology, be specifically related to a kind of Vibrio parahemolyticus flagellin monoclonal antibody, hybridoma cell strain and antigen capture ELISA test kit.
Background technology
(Vibrio parahemolyticus VP) is a kind of halophilism bacterium to Vibrio parahemolyticus.Vibrio parahaemolytisus poisoning is that feed contains due to the food of this bacterium, mainly from sea-food, as inkfish, ocean fish, extra large shrimp, sea crab, jellyfish, and contains the higher pickling food of salinity, as salted vegetables, butcher's meat etc.This bacterium survival ability is strong, can survive on rag and chopping block more than 1 month, can survive in the seawater 47 days.Be cardinal symptom with Acute onset, stomachache, vomiting, diarrhoea and watery stool clinically.This disease is many to betide the coastland in summer and autumn, often causes collective's morbidity.Owing to the seafood air transport, the inland city case also increases gradually in recent years.
At present the method that detects pathogenic microorganism in the food is mainly based on traditional method, i.e. isolation and identification method, and this method required time is long, needs 5-7 days generally speaking, reaches 10-15 days sometimes, is difficult to satisfy the needs of Rapid identification; The round pcr that grew up in recent years, be a kind of fast, sensitive, technology that specificity is good, but at present this technology still depend on traditional method before increase the bacterium step, often contain the PCR inhibitor in the enrichment liquid, thereby influence the amplification of PCR; Immunology detection based on antibody has become hazardous and noxious substances and the indispensable important technical of harmful organism detection in the food.Developed multiple specificity immunology detection technique at present, as radioimmunoassay (RIA), enzyme immunoassay (EIA), fluoroimmunoassay (FIA), time resolved fluoro-immunoassay (TrFIA), chemiluminescence immune assay (CIA), (BLIA) bioluminescence immunoassay (BIA), immunoprecipitation, immuno agglutination reaction, ELISA detection kit, immunity colloidal gold test paper strip, immune latex detection reagent etc.Multiple immunology detection technology based on antibody such as ELISA detection kit, immunity colloidal gold test paper strip wherein,, practical characteristics easy, quick, sensitive, accurate with it is the important composition in the safe detection technical system of border inspection and quarantine always, become harmful organism and hazardous and noxious substances and detected indispensable important technical.The ELISA method detects fast, as screening method have fast, sensitive characteristics, be to be subjected to the screening method of extensively welcoming, but employed test kit is expensive all from abroad, and needs its special instrument of outfit.Thereby research and development have the antibody of food-borne pathogenic microorganism of independent intellectual property right, are the exploitation ELISA detection method that has independent intellectual property right, Radioactive colloidal gold detection method, based on the basis of immune response for the immune nanometer magnetic bead enriching method on basis.
Flagellum is the important virulence factor of Vibrio parahemolyticus, has specific flagellar antigen (H antigen), one of foundation of Chang Zuowei serological identification.The flagellum of bacterium has very important physicochemical property, and its immunogenicity has great importance in biology and mechanism of causing a disease research.For example; flagellin is considered to a kind of antigen of protectiveness for the vaccine research of pathogenic bacterium; there is result of study to show; flagellin can be used as the inductor that the natural immunity is replied; induce the natural immunity of generation to reply the acquired immunity that can help to set up at exogenous antigen and reply, thereby demonstrate flagellin as the characteristic of immunological adjuvant.
In Vibrio parahemolyticus MONOCLONAL ANTIBODIES SPECIFIC FOR process before, the VP thalline of deactivation that use as antigen more, and most of albumen of thalline total albumen that is Pseudomonas, specificity between not having kind, the monoclonal antibody that causes gathering in the crops is difficult to avoid cross reaction between kind in the vibrios Pseudomonas.Specific flagellin was as antigen between this research was selected for use and had kind, and got rid of cross reaction in the positive colony screening process, the good VP monoclonal antibody of preparation specificity, and be applied to prepare Vibrio parahemolyticus ELISA detection kit.
Summary of the invention
First technical problem to be solved by this invention provides a kind of Vibrio parahemolyticus flagellin monoclonal antibody.This monoclonal antibody can be for detection of Vibrio parahemolyticus.
Second technical problem to be solved by this invention provides a kind of Vibrio parahemolyticus flagellin and catches the ELISA test kit.
For solving the problems of the technologies described above, technical scheme provided by the present invention is as follows:
Vibrio parahemolyticus flagellin monoclonal antibody provided by the present invention is to be the mouse hybridoma cell strain secretion generation of CGMCC No.6061 by deposit number.This mouse hybridoma cell strain is preserved in China Committee for Culture Collection of Microorganisms common micro-organisms center on April 26th, 2012 and (is called for short CGMCC, the address is No. 3, No. 1 institute in North Star West Road, Chaoyang District, BeiJing, China city), deposit number is CGMCC No.6061 for its deposit number.
Deposit number is that the mouse hybridoma cell strain of CGMCC No.6061 also belongs to protection scope of the present invention.
The present invention also provides a kind of Vibrio parahemolyticus flagellin to catch the ELISA test kit, and this test kit comprises the monoclonal antibody of the present invention of wrapping by the solid phase carrier of Vibrio parahemolyticus flagellin polyclonal antibody and enzyme labelling.Described enzyme is preferably horseradish peroxidase.Further, for the ease of detecting, test kit of the present invention also comprises positive control and negative control, and the required enzyme linked immunosorbent detection reagent of ELISA reaction.Wherein, described positive control is the Vibrio parahemolyticus flagellin, and described negative control is normal mouse serum or its diluent of not immune Vibrio parahemolyticus flagellin.Described enzyme linked immunosorbent detection reagent is conventional enzyme linked immunosorbent detection reagent, includes but not limited to substrate reactions liquid, washings and the reaction terminating liquid of enzyme.
The present invention has the following advantages and effect
At first, the present invention tests by specificity, comprises the non-Vibrio parahemolyticus reference culture of 30 strain Vibrio parahemolyticus and 28 strains, demonstrates good specificity and stability.Secondly, the susceptibility experimental result shows that the detection sensitivity of test kit of the present invention is 10
3/ hole apparently higher than the microorganism traditional detection method, and has advantages such as quick, efficient.
Description of drawings
Fig. 1. the SDS-PAGE figure of Vibrio parahemolyticus flagellin; Swimming lane 1: Vibrio parahemolyticus flagellin; Swimming lane 2: albumen Marker;
Fig. 2. Vibrio parahemolyticus ATCC17802 thalline and flagellum Electronic Speculum;
Fig. 3. Vibrio parahemolyticus ATCC17802 flagellin Electronic Speculum;
The SDS-PAGE figure of Fig. 4 .mAb; Swimming lane 1: albumen Marker; Swimming lane 2:mAb.
Embodiment
Method therefor is ordinary method if no special instructions among the following embodiment.
1. the extraction of yeast culture and flagellin
Vibrio parahemolyticus (Vibrio parahemolyticus) (ATCC 17802, and preserve in the laboratory) is inoculated in T1N1 substratum (available from Beijing Luqiao Technology Co., Ltd., article No. CM168), 36 ℃ of activation 24h; Picking list colony inoculation is in the TSA substratum that contains 2%NaCl (available from Beijing Luqiao Technology Co., Ltd., article No. CM417) growth 18 ~ 24h; With aseptic cotton carrier well-grown bacterium colony is uniformly coated on TSA(2%NaCl) on the substratum, cultivate 18 ± 2h for 36 ℃.Inferior daily aseptic cotton carrier is scraped in the 0.15M NaCl solution that hypothallus is suspended in precooling, ice bath 15 ~ 30min, and 1000rpm homogenate 45sec places 10min on ice immediately.The centrifugal 10min of 10000rpm under 4 ℃ of conditions of homogenate; Get the centrifugal 2h of 16000rpm under 4 ℃ of conditions of supernatant liquor, abandon supernatant, precipitation is resuspended in TET(10mM Tris, 2mM EDTA, pH8.0,1%Triton X-100) in the damping fluid.Centrifugal process repeats 3 times.Operating process keeps carrying out under the low temperature.Leave and take precipitation at last, be dissolved in a small amount of Tris-EDTA(0.1M Tris, 0.1mM EDTA, pH7.8) among the buffer, 4 ℃ of preservations are standby.
2.SDS-PAGE and Electronic Speculum is identified
The flagellin that extracts carries out the SDS-PAGE electrophoresis.5% spacer gel, 10% separation gel, 120V voltage, electrophoresis is to the glue bottom.Gel dyes with the Xylene Brilliant Cyanine G method, decolouring back gel imaging analysis systematic observation result.See Fig. 1.
Vibrio parahemolyticus thalline and single living flagellum Electronic Speculum result are as shown in Figure 2.With twice thalline of aseptic deionized water centrifuge washing, suspend, get one on copper mesh, the phospho-wolframic acid negative staining is dried, transmission electron microscope observing.The flagellin Electronic Speculum adopts same procedure, sees Fig. 3.
3. the immunity of animal
(1) immunity of BALB/c mouse
Be antigen with the flagellin, 5 of the BALB/c mouse in 6 ~ 8 ages in week of immunity are established 2 and are not done negative control as immune mouse.Initial immunity antigen add equivalent Fu Shi Freund's complete adjuvant fully emulsified after, subcutaneous injection immune mouse, 40 μ g/ mouse.Immune with same dose antigen and the fully emulsified back of freund 's incomplete adjuvant every two weeks later on.The 5th immunity tail vein blood after 3 ~ 5 days detects antiserum titre.
(2) immunity of new zealand purebred rabbit
With the female new zealand rabbit 0.5mg/ of Vibrio parahemolyticus flagellin immunity only.Every two all immunity once, be total to immunity 5 times.Five exempt from the back carried out heart in 3-5 days and measures blood greatly, put 37 ℃ 1 hour, put refrigerator then and spend the night for 4 ℃, get the serum purifying every other day and get Vibrio parahemolyticus flagellin polyclonal antibody ,-20 ℃ are frozen standby.
4. antiserum titre
Antiserum titre adopts indirect ELISA method: with PBS dilution VP antigen concentration to 1 μ g/mL, add 96 orifice plates, and 100 μ L/ holes, 4 ℃ are spent the night.Wash plate 3 times with PBST.2% bovine serum albumin is dissolved in the PBS solution, 200 μ L/ holes, 37 ℃ of sealing 1h.Wash plate with PBST.5 immune mouse serums add in the corresponding apertures with the PBS gradient dilutions, 100 μ L/ holes, and blank is PBS solution, negative control is washed plate for 37 ℃ of bags of immune serum not after by 45min.The sheep anti mouse of HRP mark adds with 1:2500 multiple dilution, 100 μ L/ holes, and 37 ℃ of bags are washed plate after by 40min.Every hole adds freshly prepared substrate solution 100 μ L, and every hole adds the 2M vitriol oil 50 μ L behind 37 ℃ of effect 15min, measures OD450nm value, reading and observations with enzyme connection detector.Tire height and satisfy the mouse of P/N value>2.0 of selection, one week the back booster immunization, get mouse boosting cell in 3 ~ 5 days and carry out cytogamy.
5.P2/0 myeloma cell's recovery and cultivation
In advance frozen myeloma cell (SP2/0) is recovered, after the quick taking-up of myeloma cell frozen in-80 ℃ of deep freezers, place 38 ℃ of water-baths slightly to rock and make its rapid thawing, notice that the frozen mouth of pipe can not run into water, in order to avoid pollute, then with cell transfer to containing 6 ~ 10ml RPMI-1640 perfect medium (RPMI-1640 substratum that contains 10% calf serum, calf serum is available from Hyclone, article No. SH30541.03) in the Tissue Culture Flask, puts into 37 ℃, 5%CO
2Cultivated in the incubator 4 ~ 6 hours, and when treating the whole adherent growth of cell, in time changed liquid, went down to posterity once every 2 ~ 3 days later on, and adjust cell and make it be in the suitableeest stand density, when cell reaches certain activity, counting is prepared to merge.Cytogamy was carried out 1 to 4 to cell in preceding 1 ~ 2 day and is gone down to posterity, and adjusting every bottle of cell concn with fresh culture is 1 ~ 2 * 10
5/ ml, the general cell that can obtain logarithmic phase in 1 ~ 2 day.
6. the preparation of feeder cell
(1) BALB/c mouse is drawn neck put to death, after the tap water flushing, be soaked in 10min in 75% alcohol fully, move in the plate of Bechtop, make its belly up.
(2) mention the mouse skin of chest abdomen with tweezers, cut off an osculum with scissors, with two tweezers skin is torn a bigger mouth, again use new tweezers then instead and mention mouse peritoneum, cut off, find the thymus gland of mouse, use tweezers, little scissors carefully takes out thymus gland, is placed in the disposable plate, and fat subsidiary on the thymus gland is peelled off in carefulness, reticular tissue etc., add the RPMI-1640 substratum (available from Hyclone, article No. SH30809.01) 5ml grinds thymus gland, sieves, thymus cell suspension is added in the centrifuge tube, the centrifugal 10min of 1000rpm abandons supernatant, twice of centrifuge washing.
(3) gently that cell is resuspended and mixed even with 5ml HAT nutrient solution, counting, adding HAT nutrient solution to cell concn is 1 ~ 2 * 10
5/ ml.
(4) cell suspension is splashed in the 96 porocyte culture plates, 37 ℃, 5%CO are put in 100 μ l/ holes (two)
2Cultivate in the incubator.
7. the preparation of immune spleen cell suspension
(1) booster immunization selected the higher BALB/c mouse of serum titer after 3 ~ 5 days, extractd eyeball, bloodletting, and collection and separation of serum are as the negative control of antibody test.
(2) disconnected neck is put to death, and is soaked in 10min in 75% alcohol after the tap water flushing, takes out mouse and is placed in the plate of aseptic Bechtop, makes its belly up.
(3) mention the mouse skin of chest abdomen with tweezers, cut off an osculum with scissors, with two tweezers skin is torn a bigger mouth again, again use new tweezers then instead and mention mouse peritoneum, cut off, find the spleen of mouse, carefully spleen is taken out, be placed in the disposable plate careful fat and the reticular tissue removed.
(4) with after the flushing of RPMI-1640 washing lotion, add new RPMI-1640 washing lotion, grind with the syringe nook closing member, sieve then, splenocyte as far as possible all is expressed in the solution by mesh, splenocyte suspension is moved in the centrifuge tube, the centrifugal 10min of 1000rpm abandons supernatant, twice of centrifuge washing.
(5) gently that splenocyte is resuspended with 10ml HAT nutrient solution, counting, standby.
The preparation of 8SP2/0 myeloma cell's suspension
(1) gets 4 bottles of cultured myeloma cells of 100ml culturing bottle (merge and change liquid the day before yesterday, cell should be in logarithmic phase during fusion), be collected in the 50ml centrifuge tube.
(2) 1000rpm is centrifugal 5 ~ 10 minutes, abandons supernatant.
(3) add 30ml RPMI-1640 washing lotion in the precipitation, resuspended gently, mixing, centrifuge washing is once again with method.
(4) gently that splenocyte is resuspended and mixed even with 10ml HAT nutrient solution, counting, standby.
9 cytogamy
(1) blow down cultured myeloma cell gently, it is transferred in the 50mL centrifuge tube, the centrifugal 7min of 1000r/min abandons supernatant, and 10mL substratum washing lotion suspends, counting.
(2) will contain 1 * 108 splenocyte suspension and contain 2 * 10
7Individual myeloma cell's suspension is mixed in the centrifuge tube of a 50ml, and the supplemented medium washing lotion is to 30ml, fully mixing.
(3) 1000rpm is centrifugal 7 minutes, and supernatant discarded cleans twice, removes supernatant as far as possible.
(4) flick centrifuge tube with have gentle hands at the bottom of, make cell mass loose evenly in the pasty state.Put 37 ℃ of water-baths, preheating 5 ~ 10min is to reach fusion temperature.
(5) 50%PEG(MW4000 that from 4 ℃ of refrigerators, takes out to have prepared), the RPMI-1640 washing lotion, be placed in 37 ℃ of water-baths, pre-temperature is standby.
(5) centrifuge tube is put in the beaker that contains 37 ~ 40 ℃ of water, rotate centrifuge tube, PEG 1ml with 1ml suction pipe absorption 50%, dropwise, slowly add centrifuge tube along tube wall, time, control was in 60 seconds, and then draw cell suspension with time of 30 seconds, and left standstill 30 seconds, in 30 seconds, cell slowly is blown in the centrifuge tube again.
(6) add the good RPMI-1640 washing lotion of pre-temperature, make the PEG dilution and lose and shortly melt effect, concrete grammar: add 2ml in preceding two minutes, added 3ml on the 3rd minute, in 3min, add 20ml at last.
(7) the centrifugal fused cell of room temperature, the centrifugal 7min of 800rpm abandons supernatant.
(8) add HAT nutrient solution (50 *, available from Sigma, article No. H0262), pressure-vaccum, resuspended sedimentation cell gently.
(9) adding of fused cell suspension is contained in 96 well culture plates of feeder cell, culture plate is put 37 ℃, 5%CO then in 100 μ l/ holes (two)
2Incubator in cultivate.
The screening of 10 positive colonies and cloning are cultivated
Merge back beginning in the 3rd day, observe each porocyte growing state every day, if pollution is arranged, handle with sodium azide immediately.Merge back 6d, 9d and change liquid with HAT nutrient solution half amount, after HAT selects nutrient solution to keep two weeks of cultivation, use instead HT(50 *, available from Sigma, article No. H0137) nutrient solution half amount is changed liquid, later on according to the cell growing state, 1 ~ 2d changes a not good liquor, uses complete culture solution instead after two weeks.Treat that hybridoma covers with (about about 10d) of hole floorage at 1/10 o'clock, draw the hole supernatant that the clone occurs and be used for specific detection.Adopt the indirect elisa method among the 1.2.3.Cross reaction: the flagellin with vibrio cholerae (VC), Vibrio vulnificus (VV) and vibrio alginolyticus (VA) is antigen, and bag is measured the cross reaction situation of VP antiserum(antisera) and 3 kinds of vibrios by 96 orifice plates.Measure OD450 with enzyme connection detector, it is positive to satisfy P/N value>2.0.VP antigen coated microplate detected result is positive, and the hybridoma that other bacterial antigens bags are negative by the plate detected result carries out cloning with limiting dilution assay and cultivates.When cell cover with the hole floorage 1/10 the time use again with quadrat method and detect, clone in the strong positive hole again.3 ~ 4 times so repeatedly, reach 100% up to the positive colony rate.
The preparation of 11 ascites is identified with antibody
The positive colony hybridoma that filters out is at last carried out enlarged culturing, and be preserved in China Committee for Culture Collection of Microorganisms common micro-organisms center on April 26th, 2012 and (be called for short CGMCC, the address is No. 3, No. 1 institute in North Star West Road, Chaoyang District, BeiJing, China city), deposit number is CGMCC No.6061.Induce method in the conventional ascites body and prepare odd contradictive hydroperitoneum.The CHARACTERISTICS IDENTIFICATION of mAb: the detection of (1) Ig class and subclass: class and subclass with Ig in the mouse mAb subclass detection kit mensuration Hybridoma Cell Culture supernatant, carry out on the operation steps by specification.(2) Western blot detects: adopt Western blot experimental technique commonly used, measure the specificity of ascites under 1: 2000 extent of dilution.(3) antibody purification and titration: ascites obtains antibody after with Protein G Sepharose affinity chromatography purifying, and the antibody behind the purifying is measured with indirect elisa method behind doubling dilution and tired.Antibody is through the SDS-PAGE purity assay.
Antibody obtains two bands clearly through the SDS-PAGE electrophoresis behind the purifying: heavy chain molecule amount 50KDa, and light chain molecular weight 25KDa, shown in Figure 4.Antibody ELISA is tired result's (seeing Table 1) as can be seen, and extent of dilution is situation under to still have very strong positive reaction at 1: 2187000.
The ELISA of table 1.mAb tires.
1. the Vibrio parahemolyticus flagellin is caught ELISA test kit composition
Having wrapped by the solid phase carrier of Vibrio parahemolyticus flagellin polyclonal antibody is enzyme plate, the Vibrio parahemolyticus flagellin monoclonal antibody of horseradish peroxidase-labeled, substrate reactions liquid, the positive and negative control, washings and the reaction terminating liquid of enzyme.
(1) the enzyme plate bag is resisted more
With the PBS damping fluid Vibrio parahemolyticus flagellin polyclonal antibody (preparing as embodiment 1) being diluted to concentration is 10 μ g/mL, wrap by the efficient desmoenzyme target of 96 hole EIA, and 100 μ L/ holes, 4 ℃ are spent the night.Take out the back and wash plate 3 times with PBST, dry.2% BSA is dissolved in the PBS solution as confining liquid, and 100 μ L/ holes add enzyme plate, 37 ℃ of sealing 1h.Take out the back and wash plate 3 times with PBST, each 3min dries, and dry final vacuum sealing is preserved.
Wherein, PBS buffered soln: Na
2HPO
412H
2O 13.76g, NaH
2PO
42H
2O 1.794g, NaCl 9g add deionized water to 1000ml; The PBST washings: contain the PBS aqueous solution of 0.005%Tween 20, PH is 7.4.
(2) mark of anti-Vibrio parahemolyticus flagellin monoclonal antibody
Adopt the periodates oxidation style to carry out coupling monoclonal antibody and the horseradish peroxidase (HRP) of anti-Vibrio parahemolyticus flagellin hybridoma cell strain CGMCC No.6061 secretion.
(3) substrate
Adopt 3,3,5,5-tetramethyl benzidine TMB(SIGMA) as the substrate of horseradish peroxidase.Sodium acetate soln (pH=4.3) 4mL, the H of adding 30%
2O
25mL, TMB 1mL, 10mL substrate reactions liquid (matching while using).
(4) positive and negative control
Positive control: by the Vibrio parahemolyticus flagellin, can extract 50 μ g/mL according to embodiment 1 described method.
Negative control: 100 times of diluents of the normal mouse serum of not immune Vibrio parahemolyticus flagellin.
(5) washings
Be the PBST washings
(6) reaction terminating liquid
2M H with the tri-distilled water preparation
2SO
4Solution.
Embodiment 3 Vibrio parahemolyticus flagellins are caught the using method of ELISA test kit
1. the processing of sample to be checked
Get sample enrichment liquid 1mL to be checked, abandon supernatant behind the centrifugal 2min of 10000rpm, precipitation adds the resuspended precipitation of a small amount of 200 μ LPBS after using PBS damping fluid washed twice.Boiling water bath 5min.
2. add contrast and sample to be checked
Get sample 100 μ L to be checked and add corresponding enzyme mark hole, a side that adds model is knocked in positive control and negative control 100 μ L/ holes, with at the bottom of guaranteeing the even coverage hole of sample, 37 ℃ hatch 1h after PBST wash plate 3 times, dry.
3. adding monoclonal antibody linked with peroxidase
Add monoclonal antibody linked with peroxidase working fluid (PBS damping fluid 1:1000 dilution enzyme mark monoclonal antibody) 100 μ L/ holes, 37 ℃ hatch 1h after PBST wash plate 3 times, dry.
4. add the substrate colour developing
Add freshly prepared tmb substrate 100 μ L/ holes, room temperature lucifuge 10 ~ 15min.
5. adding reaction terminating liquid
Add 2M H
2SO
4Solution 50 μ L/ holes, termination reaction.
6. survey the OD450nm value
Enzyme plate places microplate reader to measure the OD450nm value.
7. the result judges
As stated above, 100 times of diluents of 20 parts of negative normal mouse serum purified products are detected.According to formula threshold value=negative OD mean value+3 * standard deviation, calculating negative threshold value is 0.117.Sample OD value to be checked is judged to the positive greater than 0.117, otherwise is judged to feminine gender.
Embodiment 4 Vibrio parahemolyticus flagellins are caught specificity and the sensitivity testing of ELISA test kit
(1) specific assay
Catch the specificity of ELISA test kit in order to verify Vibrio parahemolyticus flagellin of the present invention, form and method detects 1 strain Vibrio parahemolyticus ATCC17802 and 30 strain Vibrio parahemolyticus (laboratory self-separation) and the non-Vibrio parahemolyticus reference culture of 28 strains according to embodiment 2 and embodiment 3 described test kits, see Table 2.The result shows, test kit of the present invention to Vibrio parahemolyticus ATCC17802 and 30 strain Vibrio parahemolyticus OD450nm values between 0.601 ~ 2.143, the non-Vibrio parahemolyticus reference culture of 28 strains OD450nm value between 0.065 ~ 0.091, the specificity that demonstration can be good.
Table 2
| Strain name | The OD450nm value |
| Vibrio parahemolyticus (laboratory self-separation, 30 strains) | 0.601~2.143 |
| Vibrio parahemolyticus ATCC 17802 | 2.175 |
| Vibrio cholerae 75 | 0.089 |
| Vibrio alginolyticus ATCC 1833 | 0.091 |
| Vibrio vulnificus ATCC 1758 | 0.084 |
| Ge Shi listeria spp ATCC 700545 | 0.065 |
| Xi Er listeria spp ATCC 35967 | 0.071 |
| Listeria innocua ATCC 33090 | 0.080 |
| Mo Shi listeria spp ATCC 2540 | 0.075 |
| Singly increase listeria spp ATCC 15313 | 0.078 |
| Klebsiella pneumonia CGMCC 1.1736 | 0.089 |
| Enterobacter cloacae CGMCC 1.57 | 0.090 |
| Bacillus cereus ATCC 11778 | 0.067 |
| Streptococcus aureus ATCC 25923 | 0.069 |
| Staphylococcus epidermidis ATCC 12228 | 0.075 |
| Salmonella paratyphi A CMCC 50001 | 0.084 |
| Intestinal bacteria ATCC 25912 | 0.079 |
| Rhodococcus equi ATCC 6936 | 0.069 |
| Salmonella enteritidis CMCC 50041 | 0.073 |
| Shigella flexneri CMCC 51571 | 0.088 |
| -Escherichia coli O 157 | 0.071 |
| Salmonella typhimurium CMCC 50115 | 0.084 |
| Enterobacter sakazakii ATCC 29544 | 0.078 |
| Citrobacter CMCC 48017 | 0.090 |
| The third type Hemolytic streptococcus CMCC 32206 | 0.067 |
| Beta hemolytic streptococcus CMCC 32210 | 0.074 |
| Pseudomonas aeruginosa ATCC 15442 | 0.079 |
| Yersinia entero-colitica CMCC 52212 | 0.080 |
| Shigella dysenteriae CMCC 51252 | 0.068 |
| Enterococcus faecalis CGMCC 1.2135 | 0.072 |
| Negative control | 0.087 |
(2) sensitivity testing
With Vibrio parahemolyticus ATCC17802 inoculation in the APW substratum, after 36 ℃ of shaking tables are cultivated 1h, 10 times of gradient dilutions of physiological saline, plate count simultaneously, obtaining cell concentration is 10
8~ 10
2The thalline solution of CFU/mL is formed according to embodiment 2 and embodiment 3 described test kits then and method detects, and sees Table 3.The result shows that the detection sensitivity of test kit of the present invention is 10
3/ hole.
Table 3
Obviously, the above embodiment of the present invention only is for example of the present invention clearly is described, and is not to be restriction to embodiments of the present invention.For those of ordinary skill in the field, can also make other changes in different forms on the basis of the above description.Here can't give exhaustive to all embodiments.Everyly belong to the row that apparent variation that technical scheme of the present invention extends out or change still are in protection scope of the present invention.
Claims (7)
1. Vibrio parahemolyticus flagellin monoclonal antibody is to be the hybridoma cell strain secretion generation of CGMCC No. 6061 by deposit number.
2. secretion produces the hybridoma cell strain of Vibrio parahemolyticus flagellin monoclonal antibody, and its deposit number is CGMCC No. 6061.
3. a Vibrio parahemolyticus flagellin is caught the ELISA test kit, it is characterized in that, comprises the described monoclonal antibody of claim 1 of wrapping by the solid phase carrier of Vibrio parahemolyticus flagellin polyclonal antibody and enzyme labelling.
4. test kit according to claim 3 is characterized in that, described enzyme is horseradish peroxidase.
5. according to claim 3 or 4 described test kits, it is characterized in that described test kit also comprises positive control and negative control.
6. test kit according to claim 5 is characterized in that, described positive control is the Vibrio parahemolyticus flagellin, and described negative control is normal mouse serum or its diluent of not immune Vibrio parahemolyticus flagellin.
7. the application of the described monoclonal antibody of claim 1 in the test kit of preparation detection Vibrio parahemolyticus.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201210160274 CN102659942B (en) | 2012-05-22 | 2012-05-22 | Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 201210160274 CN102659942B (en) | 2012-05-22 | 2012-05-22 | Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| CN102659942A CN102659942A (en) | 2012-09-12 |
| CN102659942B true CN102659942B (en) | 2013-09-18 |
Family
ID=46769545
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CN 201210160274 Expired - Fee Related CN102659942B (en) | 2012-05-22 | 2012-05-22 | Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit |
Country Status (1)
| Country | Link |
|---|---|
| CN (1) | CN102659942B (en) |
Families Citing this family (11)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102993301B (en) * | 2012-12-11 | 2014-02-26 | 北京出入境检验检疫局检验检疫技术中心 | Vibrio cholerae flagellin monoclonal antibody and antigen capture ELISA kit |
| CN103160602B (en) * | 2013-04-08 | 2015-07-01 | 北京出入境检验检疫局检验检疫技术中心 | Real-time fluorescent PCR (polymerase chain reaction) detection kit of vibrio parahaemolyticus and detection method thereof |
| CN103160603B (en) * | 2013-04-08 | 2014-11-19 | 北京出入境检验检疫局检验检疫技术中心 | LAMP (loop-mediated isothermal amplification) detection kit of vibrio parahaemolyticus and detection method thereof |
| CN103484434A (en) * | 2013-06-28 | 2014-01-01 | 朱艮苗 | Hybridoma cell strain and applications thereof |
| CN104316690B (en) * | 2014-11-03 | 2015-12-30 | 上海理工大学 | Vibrio parahemolyticus immune colloid gold Rapid detection test strip |
| CN104360066B (en) * | 2014-11-03 | 2016-04-13 | 上海理工大学 | Detect method and the monoclonal antibody thereof of vibrio parahemolyticus |
| CN105158470A (en) * | 2015-06-10 | 2015-12-16 | 北京农学院 | ELISA kit for detecting Vibrio parahemolyticus in aquatic product |
| CN105004866B (en) * | 2015-07-25 | 2016-08-17 | 江苏财经职业技术学院 | Quickly detect test kit and the application thereof of vibrio parahaemolyticus TDH toxin in food |
| CN105424927B (en) * | 2015-11-09 | 2017-05-10 | 山东省海洋生物研究院 | Method for detecting vibrio parahaemolyticus |
| CN110540966B (en) * | 2018-12-20 | 2023-04-28 | 湖北云璐生物工程有限公司 | Human haemophilus influenzae surface protein monoclonal antibody and antigen capture ELISA kit |
| CN113234688A (en) * | 2021-05-19 | 2021-08-10 | 上海理工大学 | Vibrio parahaemolyticus broad-spectrum colloidal gold immunochromatographic test strip, monoclonal antibody and hybridoma cell strain thereof |
Family Cites Families (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2001040280A2 (en) * | 1999-11-29 | 2001-06-07 | Inotek Corporation | Composition and method for treating a microbial infection |
| WO2003053220A2 (en) * | 2001-12-17 | 2003-07-03 | Corixa Corporation | Compositions and methods for the therapy and diagnosis of inflammatory bowel disease |
-
2012
- 2012-05-22 CN CN 201210160274 patent/CN102659942B/en not_active Expired - Fee Related
Also Published As
| Publication number | Publication date |
|---|---|
| CN102659942A (en) | 2012-09-12 |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| CN102659942B (en) | Vibrio parahaemolyticus flagellin monoclonal antibody and antigen capture ELISA (enzyme-linked immunosorbent assay) kit | |
| Tamplin et al. | Enzyme immunoassay for identification of Vibrio vulnificus in seawater, sediment, and oysters | |
| CN104789500B (en) | A kind of white diarrhea dyeing aggegation antigen and its preparation method and application | |
| KR19990022509A (en) | Culture of Lausonia Intracellularis, Anti-Lausonia Intracellulose Vaccine and Diagnostic Reagent | |
| Sithigorngul et al. | A simple and rapid immunochromatographic test strip for detection of pathogenic isolates of Vibrio harveyi | |
| CN106834235A (en) | Anti- Tilapia mossambica IgM monoclonal antibody cell line and its screening technique and application | |
| CN103160604A (en) | LAMP (loop-mediated isothermal amplification) detection kit for Vibrio vulnificus and detection method using same | |
| CN104316690A (en) | Rapid vibrio parahaemolyticus immune colloidal gold test strip | |
| Milder et al. | Comparison of histological and immunological techniques for detection of Pneumocystis carinii in rat bronchial lavage fluid | |
| CN102993301B (en) | Vibrio cholerae flagellin monoclonal antibody and antigen capture ELISA kit | |
| Pengsuk et al. | Differentiation among the Vibrio cholerae serotypes O1, O139, O141 and non-O1, non-O139, non-O141 using specific monoclonal antibodies with dot blotting | |
| CN104312979A (en) | Anti-H7 subtype avian influenza virus monoclonal antibody and application thereof | |
| CN104774782B (en) | Chicken source enterococcus faecalis separation strains and its application | |
| Varavithya et al. | Importance of Salmonellae and Campylobacter jejuni in the etiology of diarrheal disease among children less than 5 years of age in a community in Bangkok, Thailand | |
| CN103044545B (en) | Vibrio vulnificus flagellin monoclonal antibody and antigen capture ELISA (Enzyme Linked Immunosorbent Assay) kit | |
| CN103160606B (en) | LAMP (loop-mediated isothermal amplification) detection kit of vibrio cholerae and detection method thereof | |
| AU603774B2 (en) | Specific mycoplasma membrane antigen and antibody and their clinical applications | |
| Phianphak et al. | Production of monoclonal antibodiesfor detection of Vibrio harveyi | |
| CN105543177A (en) | Hybridoma cell strain secreting citrus yellow vein clearing virus-resistant monoclonal antibodies and monoclonal antibody application thereof | |
| CN102220285A (en) | Monoclonal antibody of outer membrane protein of chlamydia abortus and application thereof | |
| CN104789499B (en) | A kind of white diarrhea agp antigen and its preparation method and application | |
| CN103160601B (en) | Real-time fluorescent PCR (polymerase chain reaction) detection kit for Vibrio vulnificus and detection method using same | |
| CN101205528B (en) | Spiro protomer strain and uses thereof | |
| CN105132282B (en) | Campylobacter jejuni immuno-PCR detection kit | |
| WO2012016107A1 (en) | Methods and kits for detection of salmonella enteritidis and related serovars |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| C06 | Publication | ||
| PB01 | Publication | ||
| C10 | Entry into substantive examination | ||
| SE01 | Entry into force of request for substantive examination | ||
| C14 | Grant of patent or utility model | ||
| GR01 | Patent grant | ||
| CF01 | Termination of patent right due to non-payment of annual fee |
Granted publication date: 20130918 Termination date: 20210522 |
|
| CF01 | Termination of patent right due to non-payment of annual fee |