A kind of detection kit and application of African swine fever virus antibody based on chimeric p54 epitope
An African swine fever virus and antibody detection technology, applied in accurate detection, specificity of African swine fever virus P54 antibody, blocking ELISA kit, rapid field, can solve problems such as sensitivity and specificity limitations, and achieve improved sensitivity The effect of sex and specificity, avoiding the risk of viral spread
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example 1
[0102] Example 1 Structural Analysis of Bluetongue Virus VP7 Protein and Prediction of Flexible Structure Region
[0103] Bluetongue virus core-like particles are assembled from bluetongue virus structural proteins VP3 and VP7, and 60 VP3 dimers (120 VP3 proteins) assemble to form the inner core of core-like particles with a diameter of 55 nm, and 260 VP7 three Aggregates (780 VP7 proteins) are located in the outer layer of core-like particles similar to a brush coat, and the structure is as follows: figure 1 . For this reason, the present invention takes VP7 protein as the transformation target.
[0104] The invention adopts tools such as Garnier-Robson method, Chou-Fasman method and Karplus-Schulz method to analyze the structure of the bluetongue virus VP7 protein, so as to predict the flexible structural region of the VP7 protein. Finally, the present invention screened out 8 possible flexible structural regions, and their positions and amino acid residue sequences are sh...
example 2
[0107] Example 2 The bluetongue virus VP7 amino acid sequence of the chimeric African swine fever virus P54 epitope
[0108] The research team analyzed the secondary structure of the African swine fever virus P54 protein and determined that 66EDIQFINPYQ75 in the amino acid sequence of the P54 protein is a conserved epitope. According to NCBI comparison analysis, almost all African swine fever virus P54 proteins contain this amino acid sequence; And the research team screened and prepared a monoclonal antibody against this epitope (P54-2E4 MAb). For this reason, the present invention replaces the 8 possible flexible structural regions of the bluetongue virus VP7 protein in case 1 with the EDIQFINPYQ amino acid sequence, thereby obtaining the bluetongue virus VP7 amino acids of 8 chimeric African swine fever virus P54 antigenic epitopes Sequence, see Table 2 for specific alternatives
[0109] Table 2 Alternatives
[0110]
example 3
[0111] Example 3 Preparation and identification of chimeric core-like particles
[0112] (1) Construction of recombinant baculovirus
[0113] Insert the bluetongue virus vp3 gene into the vector pFastBac by gene synthesis and subcloning technology TM Dual, construct the recombinant plasmid pFastBac-Dual-vp3; then the VP7 gene (rvp7(47-51), rvp7(78-84), rvp7(113-119), rvp7(136-142), rvp7(155) after mutation -161), rvp7(175-179), rvp7(182-188)) and rvp7(233-239) were respectively inserted into another multiple cloning site of the vector, thereby constructing and obtaining 8 kinds of recombinant plasmids pFastBac-Dual- vp3-rvp7(47-51), pFastBac-Dual-vp3-rvp7(78-84), pFastBac-Dual-vp3-rvp7(113-119), pFastBac-Dual-vp3-rvp7(136-142)pFastBac-Dual - vp3-rvp7(155-161), pFastBac-Dual-vp3-rvp7(175-179), pFastBac-Dual-vp3-rvp7(182-188) and pFastBac-Dual-vp3-rvp7(233-239). The recombinant plasmids with correct sequencing were transformed into DH10Bac, screened by blue-white spot and co...
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