CN106191304A - Immunomagnetic beads test kit of detection PPR virus antigen and application thereof - Google Patents

Immunomagnetic beads test kit of detection PPR virus antigen and application thereof Download PDF

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CN106191304A
CN106191304A CN201610537118.7A CN201610537118A CN106191304A CN 106191304 A CN106191304 A CN 106191304A CN 201610537118 A CN201610537118 A CN 201610537118A CN 106191304 A CN106191304 A CN 106191304A
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immunomagnetic beads
pprv
test kit
pbs
protein
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CN106191304B (en
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吴锦艳
尚佑军
张志东
陈妍
王光祥
刘湘涛
尹双辉
�田宏
杨顺利
刘永军
张克山
栾志舫
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Inner Mongolia Hetao Agriculture And Animal Husbandry Technology Research Institute
Lanzhou Veterinary Research Institute of CAAS
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Lanzhou Veterinary Research Institute of CAAS
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Abstract

The invention discloses a kind of immunomagnetic beads test kit detecting PPR virus antigen and application thereof, belong to biological technical field.Test kit of the present invention includes the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling, is the primer pair that target spot detects PPR virus antigen with PPRVM genetic fragment, RT PCR reaction mixture and RNA polymerase.The sequence of described primer pair is respectively as shown in SEQ ID NO.1 and SEQ ID NO.2.During the proposition of the present invention overcomes PPR virus Detection of antigen, PPRV cause of disease is degradable, and the venom finite volume to be checked used during the extraction of cause of disease RNA causes extracted RNA to be unable to reach the minimum requirements of RT PCR detection, and the problem of false negative result occurs, the detection for PPR virus antigen provides a kind of effective technological means.

Description

Immunomagnetic beads test kit of detection PPR virus antigen and application thereof
Technical field
The present invention relates to a kind of immunomagnetic beads test kit and application thereof, be used for detecting PPR particularly to one sick Immunomagnetic beads test kit of poison antigen and application thereof, the invention belongs to biological technical field.
Background technology
Also known as sheep pestilence, main infection is little ruminates beast to PPR (Peste des petits runinants, PPR), Particularly goat and sheep is the most susceptible, and also even in wild animal have generation, is by PPR virus (Peste des Petits runinants virus, PPRV) a kind of serious acute, strong, the high degree in contact infectious disease that cause, at present There is no the report infecting people, its M & M Gao Jun is up to 100%, and world animal health group (OIE) is classified as The animal epidemic of statutory report, China is also classified as a class animal epidemic." national medium-term and long-term animal epidemic control program One of (2012-2020) " the 13 kinds of exotic animals epidemic diseases being classified as guard key.At present, PPR is entirely State's most area is even has generation, serious threat animal health safety and the development of China's animal husbandry of China, is to need sternly Lattice are taked to force one of prevention and control and animal epidemic of putting out.
Immunomagnetic bead technique (Immunomagnetic beads, IMB) is a kind of based on antigen antibody reaction, with magnetic Carrier technique is the new diagnostic technology of medium.Due to spies such as it are distinctive quickly, efficient, low toxicity, specificity are high, simple to operate Put and be widely used at biomedical sector.Jacobsen utilizes Lee of immunomagnetic bead technique detection monocyte hyperplasia This special Salmonella, its sensitivity can detect that the 3x10 in culture fluid4Individual bacterium, the response rate is 95%, permissible in mixed-culture medium Well go unless purpose bacterium, and specificity is good.Yang Wan etc. establish a kind of immuno magnetic cell separation technical tie-up real-time quantitative The method of rotavirus in PCR Quantitative detection water, and the specific immune magnetic of rotavirus in water can be separated by preparation Pearl, is used successfully to the detection of rotavirus in water.Yan little Fei etc. use immuno magnetic cell separation technology and impedance measurement technique combination Method, it is achieved that the specificity of bird flu H5 subtype virus is quickly detected.He Jingyun etc. utilize specific antibody to be coated magnetic Pearl, has successfully been enriched with purification Clostridium piliformis from infected rats liver, and result of study shows, immuno magnetic cell separation skill Art can efficiently separate and purification Clostridium piliformis, checks that inapparent infection provides new approaches for Serological Antigens.
The conventional sense infected for PPRV and diagnostic method are a lot, and the standard detecting method that OIE specifies is competition ELISA and RT-PCR method.Wherein competitive ELISA is mainly as the Serology test of PPRV antibody, owing to cannot be distinguished by Differentiating vaccine immunity antibody and natural infection antibody, therefore the infection at PPRV is finally made a definite diagnosis in detecting and be need nonetheless remain for coordinating PCR Diagnostic antigen judge whether occur PPRV infect.PPRV is sub-thread minus-stranded rna virus, to external world environment sensitive, 50 DEG C, 30min or sunlight will soon inactivate degraded under irradiating.Owing to PCR detection cannot be carried out in the wild, therefore in pathological material of disease collection and Easily cause viral level in tissue pathological material of disease during preservation to reduce, to such an extent as to cause false-negative testing result.
M albumen is one of PPRV major structural protein, plays during intracellular release in ripe virion Pivotal role, in the case of disappearance M albumen, virus will lose the ability of infection cell, and currently for PPRV M gene Detection method little, the present invention is directed to the detection for PPRV of the PPRV M gene design primer, as the target of PCR method detection Mark gene, found that the primer sensitivity of present invention design is high, specificity is good, simultaneously because the virus enrichment of immunomagnetic beads is made With, therefore can effectively solve the low problem being difficult to detect of viral level in PPR virus Detection of antigen, can be effective The cause of disease detector efficiency of increase PCR method.
Summary of the invention
For degradable due to PPRV cause of disease during PPR virus Detection of antigen present in prior art, and The venom finite volume to be checked that cause of disease RNA uses during extracting causes extracted RNA to be unable to reach RT-PCR detection Low requirement, and the problem of false negative result occurs, one aspect of the present invention devises a pair can be used for PRRVM gene as target spot The specific primer of PPRV detection, is on the other hand prepared for a kind of specific immunity magnetic bead that can be used for being enriched with PPRV cause of disease, and Finally establish a kind of immunomagnetic beads test kit that can be used for detecting PPR virus antigen.
Concrete, in order to achieve the above object, present invention employs techniques below means:
A kind of immunomagnetic beads test kit for detecting PPR virus antigen of the present invention, it includes the anti-PPRV of rabbit The immunomagnetic beads of H protein IgG coupling, take PPRV M genetic fragment as the primer pair of target spot detection PPR virus antigen, RT-PCR reaction mixture and RNA polymerase, the sequence of described primer pair is respectively such as SEQ ID NO.1 and SEQ ID Shown in NO.2.
In the present invention, it is preferred to, the concentration of the immunomagnetic beads of described rabbit anti-PPRV H protein IgG coupling is 10mg/ mL。
In the present invention, it is preferred to, described immunomagnetic beads test kit also includes PBS, preferred described PBS is 10mM, pH value is the PBS of 7.4.
In the present invention, it is preferred to, the immunomagnetic beads of described rabbit anti-PPRV H protein IgG coupling is by the following method Prepare:
1) washing of magnetic bead: take magnetic bead stock solution in EP pipe in, utilize magnetic frame adsorption, with PBS washing 3 Secondary, finally resuspended with PBS;
2) coupling of antibody: by excess rabbit anti-PPRV H protein IgG antibody join step 1) resuspended after magnetic bead in, Mixing, 37 DEG C of concussion 15-60min, obtain the suspension of immunomagnetic beads containing rabbit anti-PPRV H protein IgG coupling;
3) separation of the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling: by step 2) suspension that obtains utilizes magnetic force Frame adsorbs, and removes supernatant, washs 3 times with PBS, finally resuspended with PBS, i.e. obtains required rabbit anti-PPRV H The immunomagnetic beads of protein I gG coupling.
In wherein, it is preferred that step 1), the volume of magnetic bead stock solution is 200 μ L, and the weight of magnetic bead contained therein is 6mg, Use 600 μ LPBS buffer resuspended;Step 2) described in the consumption of rabbit anti-PPRV H protein IgG antibody be 100 more than μ g.
Wherein, it is preferred that step 1) and step 3) described in PBS be 10mM, pH value be 7.4 PBS delay Rush liquid.
The concussion time in wherein, it is preferred that step 2) is 20min.
Wherein, it is preferred that the final concentration of 10mg/mL of the immunomagnetic beads of described rabbit anti-PPRV H protein IgG coupling.
Further, the invention also discloses described immunomagnetic beads test kit in detection PPR virus antigen Purposes.
When using immunomagnetic beads test kit of the present invention for detecting PPR virus antigen, according to following step Suddenly carry out:
1) enrichment of virus: take immunomagnetic beads in the EP pipe of 1.5mL, adds sample to be checked, 37 DEG C of concussion reaction 20- 60min;
2) washing of magnetic bead: after virus has been enriched with, EP pipe is positioned on magnetic frame, supernatant discarded, buffers with PBS Liquid washs 3 times, adds the PBS of 2-5 times of volume by resuspended for the immunomagnetic beads of enriching virus;
3) extraction of viral RNA: with pyrolysis method break virus structure, releasing virus RNA;
4) PCR amplification: utilize test kit of the present invention to carry out the amplification of One step RT-PCR;
5) the 1% analysing amplified result of agarose gel electrophoresis.
The immunomagnetic beads amount used during each 400 μ L measuring samples detection in wherein, it is preferred that step 1) is 20 μ L, 37 DEG C concussion the response time be 30min;Step 2) in use pyrolysis method obtain viral RNA program be: 95 DEG C cracking 10min Rear ice bath 3min rapidly;Step 3) in the amplification reaction system of One step RT-PCR be: PrimeScript 1Step Enzyme Mix 2μL;2×1Step Buffer 25μL;PPRV RNA template 6 μ L;RNase Free dH2O 15μL;Forward primer 1 μ L;Downstream primer 1 μ L, cumulative volume 50 μ L.
Amplification program is: 50 DEG C of 30min;94℃3min;94 DEG C of degeneration 30s, 57 DEG C of renaturation 30s, 72 DEG C extend 1min, altogether Carry out 35 circulations;In 4 DEG C of preservations after 72 DEG C of extension 10min.
During the proposition of the present invention overcomes PPR virus Detection of antigen, PPRV cause of disease is degradable, and cause of disease The venom finite volume to be checked that RNA uses during extracting causes extracted RNA to be unable to reach the minimum of RT-PCR detection will Asking, and the problem of false negative result occur, the detection for PPR virus antigen provides a kind of effective technological means.
Accompanying drawing explanation
Fig. 1 is the purification of rabbit anti-PPRV H protein serum IgG;
M: pre-dsred protein Marker;1: eluent 1;2: eluent 2;3: eluent 3;
Fig. 2 is the specific result of immunomagnetic beads by SDS-PAGE detection rabbit anti-PPRV H protein IgG coupling;
1: combine the product after PPRV-H albumen;2:PPRV-H albumen former state;3: combine the product of PPRV vaccine diluent: 4:PPRV vaccine diluent;
Fig. 3 is RT-PCR amplification;
M:DNA Marker DL2000;1-5:PPRV RNA amplification result;6: negative control
Fig. 4 be rabbit anti-PPRV H protein IgG coupling immunomagnetic beads enrichment after carry out RT-PCR amplification (sensitivity examine Survey).
M:DNA Marker DL2000;1: negative control;2:3mL vaccine diluent;3:2mL vaccine diluent;4-9: 1mL takes turns doing the vaccine diluent after ten times of doubling dilutions.
Detailed description of the invention
Below in conjunction with specific embodiment further describe the present invention, advantages of the present invention and feature will be with describe and Apparent.But embodiment is merely to illustrate the present invention, protection scope of the present invention is not constituted any restriction.This area skill Art personnel it should be understood that can be to the details of technical solution of the present invention and shape under without departing from the spirit and scope of the present invention Formula is modified or replaces, but these amendments and replacement each fall within protection scope of the present invention.
Embodiment 1 is with PPRV M genetic fragment as target spot, for detecting the primer pair of PPR virus antigen Design and synthesis
Inventor according to PPRV Nigeria 75/1 strain whole genome sequence in GenBank (accession number: HQ197753.1) design is for the specific primer pair of M gene, and the sequence of described primer pair is as follows:
Forward primer 1-up:ATGACCGAGATCTACGATT (shown in SEQ ID NO.1);
Downstream primer 1-low:ACAGGATCTTGAACAGGCC (shown in SEQ ID NO.2).
Described primer synthesizes transferring to biotech firm.
The preparation of embodiment 2 rabbit anti-PPRV H protein hyper-immune serum
Design according to PPRV Nigeria 75/1 strain whole genome sequence (accession number: HQ197753.1) in GenBank For the specific primer of H gene, primer is synthesized by biotech firm.Primer sequence is as follows:
Shown in PPRV-H up:5'-CGGGATCCATGTCCGCACAAAGGGAA-3'(SEQ ID NO.3)
Shown in PPRV-H down::5'-ATTTGCGGCCGCTCAGACTGGATTACATGTTA-3'(SEQ ID NO.4)
With PPR virus vaccine (vaccine is purchased from Xinjiang Tiankang Raise Livestock Biotechnology Co., Ltd) as masterplate Amplification obtains H gene, obtains H protein by prokaryotic expression purification.
Choose the healthy adult male rabbit (new zealand white rabbit) 10 of body weight about about 2kg, nape portion multiple spot and after PPRV H protein after limb femoribus internus subcutaneous inoculation Prokaryotic expression, purification.
Concrete immune programme for children: head exempts from front rabbit ear edge vein exploitating blood redundant detection, Freund's complete adjuvant and mesh during immunity Albumen mixed in equal amounts after carry out emulsifying by emulsator, immunizing dose is every rabbit about 5mg;Head exempts from rear 2 weeks auricular veins Blood sampling detection antibody horizontal, carries out booster immunization, and immunizing dose increases to every rabbit about 10mg;Two exempt from after the 2nd week, the 3rd Taking a blood sample respectively in week and carry out antibody test, when antibody titer reaches the highest beginning to decline, carry out three and exempt from, immunity amount exempts from phase with two With;Three exempt from one week after blood sampling detection antibody titer, if ELISA method detection titer reaches 1:6400, then by Culling heart blood, obtain Obtain rabbit anti-PPRV H protein hyper-immune serum.
The preparation of the immunomagnetic beads of embodiment 3 rabbit anti-PPRV H protein IgG coupling
(1) purification of rabbit anti-PPRV H protein hyper-immune serum IgG:
Pharmacia Corp of Sweden AKTA FPLC protein purification system concrete operation step:
1) the transfusion entrance (A, B) of instrument is respectively put in corresponding required buffer, opens computer, select UNICORN Software, in system control interface, selects " manual pump wash FPLC " to select the entrance A used, performs function and rinse The pipeline of purification system and pump;
2) G-protein affinity chromatograph protein purification post is connected;
3) system is arranged: in system control interface, selects " manual pump Flow " input flow velocity, " insert Alarm&mon alarm pressure " in the pressure of front pump;
4) balance purification column: with the pH of the Tris-HCl buffer balance purification column of 1M pH 9.0;
5) loading: after the rabbit anteserum distilled water of PPRV H protein immunity is done 1:5 dilution, adds in sample-adding pipe The conductance of 10mL, Binding Buffer controls at 50-60mS/cm, pH 7.0-7.4, and flow velocity is 1.0mL/min, flows through about About 0.5h, collects and flows through liquid, and every 2ml collects 1 pipe.
6) eluting: after peak to be absorbed is stable, the pH adding Elution Buffer, Elution Buffer controls at 2.5- About 3.0, flow velocity is 1.0mL/min, observes absworption peak, rises time control sample receiver rapidly at absworption peak and receives eluting Liquid, when collecting eluent, every 2mL collects a pipe, the most named eluent 1, eluent 2 ... add pH after collection immediately In the Tris-HCl buffer of 9.0 and the pH of eluent so that it is pH is maintained at neutrality or alkalescence.
7) after eluting, first with distilled water flushing pump and pipeline, then continue to rinse with 20% ethanol.
8) measure the IgG concentration of recovery purification with NanoDrop2000A280, and run SDS-PAGE analysis IgG after purification Purity, purification effect figure is shown in Fig. 1.
(2) preparation of the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling
1) washing of magnetic bead: take 200 μ L (about 6mg) magnetic bead stock solution (purchased from life biotech firm) in EP manage in, utilize magnetic Power frame adsorption, washs 3 times with PBS, finally resuspended with 600 μ L PBS.
2) coupling of antibody: the anti-PPRV H protein IgG antibody (more than 100 μ g) of excess is joined step 1) obtain In magnetic bead suspension, mixing, 37 DEG C of concussion 20min, obtain the suspendible of immunomagnetic beads containing rabbit anti-PPRV H protein IgG coupling Liquid;
3) separation of the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling: by step 2) suspension that obtains utilizes magnetic force Frame adsorbs, and removes supernatant, washs 3 times with PBS, finally resuspended with PBS, i.e. obtains required rabbit anti-PPRV H The immunomagnetic beads of protein I gG coupling, its concentration is 10mg/mL.
Wherein, PBS used is 10mM, pH value is the PBS of 7.4.
(3) specific detection of rabbit anti-PPRV H protein IgG coupling immunomagnetic beads:
1) take immunomagnetic beads that 50 μ L prepare respectively in the EP of 3 1.5mL manages, be separately added into 200 μ L unpurified PPRV H protein and 1:10 times dilute after PPR live vaccine (vaccine is purchased from Xinjiang Tian Kang herding biotechnology share Company limited, viral level is about 104TCID50/mL).Inhaling with liquid-transfering gun and play mixing, 37 DEG C of reaction 2h or 4 DEG C of reactions are overnight (anti- During Ying, irregular liquid-transfering gun mixes);
2) after fully reacting, take out EP pipe, be placed on magnetic frame absorption 2min, with liquid-transfering gun by complete for supernatant sucking-off;
3) taking off EP pipe from magnetic frame, the PBS adding 1mL pH 7.4 rinses, and fully after mixing, reapposes in magnetic Adsorbing 2min on power frame, with liquid-transfering gun by whole for supernatant sucking-offs, such repeated washing 3-5 time, finally with 200 μ L pH's 7.4 PBS is resuspended by magnetic bead, draws part suspension, adds 4 × protein electrophoresis sample-loading buffer, does not boils, directly carry out SDS-PAGE Electrophoretic analysis, result is shown in Fig. 2, and this result illustrates, this immunomagnetic beads can be good at combining PPRV H protein and PPRV is the most sick Poison.
Embodiment 4 is for detecting the preparation of the immunomagnetic beads test kit of PPR virus antigen
Described test kit includes that (10mg/mL, embodiment 2 is made for the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling Standby), with PPRVM genetic fragment be target spot detection PPR virus antigen primer to (50pM) (respectively such as SEQ ID Shown in NO.1 and shown in SEQ ID NO.2), PBS (10mM, pH value are 7.4), 2 × 1Step Buffer and PrimeScript 1Step Enzyme Mix。
The test kit of embodiment 5 present invention purposes in detection PPR virus antigen
1, detection sample
1:10 times dilute after PPR virus vaccine.(vaccine has purchased from Xinjiang Tian Kang herding biotechnology share Limit company, viral level is about 104TCID50/mL)
2, method
1) enrichment of virus: take immunomagnetic beads (10mg/mL) the 20 μ L of rabbit anti-PPRV H protein IgG coupling in 1.5mL's In EP pipe, add the PPR virus vaccine after 400 μ L dilutions, 37 DEG C of concussion reaction 30min;
2) washing of magnetic bead: after virus has been enriched with, EP pipe is positioned on magnetic frame, supernatant discarded, buffers with PBS Liquid washs 3 times, adds 1.2ml PBS (10mM, pH value are 7.4) by resuspended for the immunomagnetic beads of enriching virus;
3) extraction of viral RNA: with pyrolysis method break virus structure, releasing virus RNA;Pyrolysis method obtains virus The program of RNA is: rapid ice bath 3min after 95 DEG C of cracking 10min;
4) PCR amplification: utilize the test kit described in embodiment 4 to carry out the amplification of One step RT-PCR;
The amplification reaction system of One step RT-PCR is:
Amplification program is as follows:
5) the 1% analysing amplified result of agarose gel electrophoresis.
Having carried out 5 repetitions altogether, result is as it is shown on figure 3, this result shows, the test kit using the present invention can be the most right PPR virus expands, and repeatability is good.
Embodiment 6: the sensitivity test of the test kit of the present invention
PPR virus vaccine 1:10 times dilute after (viral level is about 103TCID50/ mL), take 1mL viral dilution Liquid does ten times of doubling dilutions, and respectively 100、10-1、10-2、10-3、10-4、10-5, add respectively 3mL, 2mL vaccine dilution stock solution and 1mL 100、10-1、10-2、10-3、10-4、10-5Ten times of doubling dilution liquid of vaccine are through the immune magnetic of rabbit anti-PPRV H protein IgG coupling Pearl enrichment after, extract virus genome RNA, carry out RT-PCR, method with embodiment 5, result such as Fig. 4.Result shows, uses this The minimum sample virus concentration detected of method of invention is 0.1TCID50/mL。

Claims (10)

1. the immunomagnetic beads test kit detecting PPR virus antigen, it is characterised in that described test kit includes rabbit The immunomagnetic beads of anti-PPRV H protein IgG coupling, with PPRVM genetic fragment drawing for target spot detection PPR virus antigen Thing pair, RT-PCR reaction mixture and RNA polymerase, the sequence of described primer pair is respectively such as SEQ ID NO.1 and SEQ ID Shown in NO.2.
2. immunomagnetic beads test kit as claimed in claim 1, it is characterised in that also include in described test kit that PBS buffers Liquid, it is preferred that described PBS is 10mM, pH value is the PBS of 7.4.
3. immunomagnetic beads test kit as claimed in claim 1, it is characterised in that the anti-PPRV H protein IgG coupling of described rabbit The concentration of immunomagnetic beads is 10mg/mL.
4. immunomagnetic beads test kit as claimed in claim 1, it is characterised in that the anti-PPRV H protein IgG coupling of described rabbit Immunomagnetic beads is prepared by the following method and obtains:
1) washing of magnetic bead: take magnetic bead stock solution in EP pipe, utilize magnetic frame adsorption, with PBS washing 3 times, Resuspended with PBS afterwards;
2) coupling of antibody: the rabbit anti-PPRV H protein IgG antibody of excess is joined step 1) resuspended after magnetic bead in, mixed Even, 37 DEG C of concussion 15-60min, obtain the suspension of immunomagnetic beads containing rabbit anti-PPRV H protein IgG coupling;
3) separation of the immunomagnetic beads of rabbit anti-PPRV H protein IgG coupling: by step 2) suspension that obtains utilizes magnetic frame to inhale Attached, remove supernatant, wash 3 times with PBS, finally resuspended with PBS, i.e. obtain required rabbit anti-PPRV H protein The immunomagnetic beads of IgG coupling.
5. immunomagnetic beads test kit as claimed in claim 4, it is characterised in that step 1) in the volume of magnetic bead stock solution be 200 μ L, the weight of magnetic bead contained therein is 6mg, uses 600 μ L PBS resuspended;Step 2) described in rabbit anti-PPRV H The consumption of protein I gG antibody is 100 more than μ g.
6. immunomagnetic beads test kit as claimed in claim 4, it is characterised in that step 1) and step 3) described in PBS delay Rush liquid be 10mM, pH value be the PBS of 7.4.
7. immunomagnetic beads test kit as claimed in claim 4, it is characterised in that step 2) in the concussion time be 20min.
8. immunomagnetic beads test kit as claimed in claim 4, it is characterised in that the anti-PPRV H protein IgG coupling of described rabbit The final concentration of 10mg/mL of immunomagnetic beads.
9. the immunomagnetic beads test kit as described in any one of claim 1-8, it is characterised in that be used for detecting PPR sick During poison antigen, follow the steps below:
1) enrichment of virus: take immunomagnetic beads in the EP pipe of 1.5mL, adds sample to be checked, 37 DEG C of concussion reaction 20-60min;
2) washing of magnetic bead: after virus has been enriched with, EP pipe is positioned on magnetic frame, supernatant discarded, washes with PBS Wash 3 times, add the PBS of 2-5 times of volume by resuspended for the immunomagnetic beads of enriching virus;
3) extraction of viral RNA: with pyrolysis method break virus structure, releasing virus RNA;
4) PCR amplification: utilize the test kit described in claim 1 to carry out the amplification of One step RT-PCR;
5) the 1% analysing amplified result of agarose gel electrophoresis.
10. immunomagnetic beads test kit as claimed in claim 9, it is characterised in that step 1) in every 400 μ L measuring samples detections Time use immunomagnetic beads amount be 20 μ L, 37 DEG C concussion the response time be 30min;Step 2) the middle pyrolysis method acquisition disease used The program of poison RNA is: rapid ice bath 3min after 95 DEG C of cracking 10min;Step 3) in the amplification reaction system of One step RT-PCR For: PrimeScript 1 Step Enzyme Mix 2 μ L;2×1 Step Buffer 25μL;PPRV RNA template 6 μ L; RNase Free dH2O 15μL;Forward primer 1 μ L;Downstream primer 1 μ L, cumulative volume 50 μ L;
Amplification program is: 50 DEG C of 30min;94℃ 3min;94 DEG C of degeneration 30s, 57 DEG C of renaturation 30s, 72 DEG C extend 1min, enter altogether Row 35 circulation;In 4 DEG C of preservations after 72 DEG C of extension 10min.
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CN110373501A (en) * 2019-08-02 2019-10-25 中国农业科学院兰州兽医研究所 A kind of Porcine epidemic diarrhea virus quick detection kit based on biomolecular

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