Porcine pseudorabies virus gene deletion strain and vaccine composition and preparation method and application thereof
A technique for porcine pseudorabies virus and vaccine composition, applied in the field of animal virology
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Embodiment 1
[0069] Embodiment 1, the preparation of PRV HN1201 strain UL21 deletion strain
[0070] 1.1 Construction of PRV HN1201GFP recombinant virus transfer vector
[0071] According to the sequence of the UL21 gene to be deleted, design homology arms at its two ends, respectively UL21A and UL21B. UL21A and UL21B were cloned into pUC19 vector and named pUCUL21AB. Then the GFP gene was cloned into pUCUL21AB to obtain a recombinant virus transfer vector, which was named pUCUL21A-GFP-B. The homology arms in the transfer vector are the sequences on both sides of UL21, so the recombinant virus obtained after recombination is the deletion of the UL21 gene. The schematic diagram of recombinant transfer vector construction is shown in figure 1 , figure 2 is the location of the UL21A and UL21B homology arms on the genome.
[0072] 1.1.1. Amplification and cloning of homologous recombination arm
[0073] 1.1.1.1 Primer design and template preparation
[0074] According to the gene seque...
Embodiment 2
[0115] Embodiment 2, the preparation of PRV HN1201 strain TK / gE / gI / deletion strain
[0116] 1. Preparation of TK deletion strain
[0117] 1.1 Construction of GFP intermediate transfer vector required for deletion of PRV HN1201TK
[0118] According to the sequence of the TK gene to be deleted, design homology arms at its two ends, respectively TKA and TKB. TKA and TKB were cloned into pUC19 vector, named pUCTKAB. Then the GFP gene was cloned into pUCTKAB to obtain the recombinant virus transfer vector, which was named pUCTKA-GFP-B. The homologous arms in the transfer vector are sequences on both sides of TK, so the recombinant virus obtained after recombination is a virus with TK gene deletion. Figure 4 It is a schematic diagram of the deletion position of the TK gene and the position of the TKA and TKB homology arms on the genome.
[0119] 1.1.1. Amplification and cloning of homologous recombination arm
[0120] 1.1.1.1 Primer design and template preparation
[0121] A...
Embodiment 3
[0207] Example 3 Preparation of PRV HN1201TK- / gE- / gI- / UL21-deleted strain
[0208] 3.1 Construction of GFP intermediate transfer vector required for deletion of UL21 in PRV HN1201
[0209] Prepare PRV HN1201TK with embodiment 2 - / gE - / gI - strain. According to the sequence of the UL21 gene to be deleted, design homology arms at its two ends, respectively UL21A and UL21B. UL21A and UL21B were cloned into pUC19 vector and named pUCUL21AB. Then the GFP gene was cloned into pUCUL21AB to obtain a recombinant virus transfer vector, which was named pUCUL21A-GFP-B. The homology arms in the transfer vector are the sequences on both sides of UL21, so the recombinant virus obtained after recombination is the deletion of the UL21 gene. The schematic diagram of recombinant transfer vector construction is shown in figure 1 , figure 2 is the location of the UL21A and UL21B homology arms on the genome.
[0210] 3.1.1. Amplification and cloning of homologous recombination arm
[0...
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