Pseudorabies TK*/gE*/gI* gene dificiency mark live vaccine and preparation method thereof
A gene deletion vaccine and pseudorabies virus technology, applied in the field of animal virology, can solve the problems of unclear side effects, deletion, g1/gp63 insertion inactivation sequence, etc.
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[0050] 1. Construction of pseudorabies virus gE, gI double gene deletion transfer vector pFBBS:
[0051] Plasmid pSKFB was double-digested with BstE II and Stu I, the 1247bp fragment was discarded, and the 5.7kb fragment was recovered, filled in with Klenow enzyme, and ligated with T4DNA ligase to obtain a recombinant plasmid. The plasmid contains part of the gD gene, part of the gI gene, part of the gE gene, all of the 11K gene and part of the 28K gene, and is named pFBBS. Using pFBBS as a template and P7 and P8 as primers for PCR, a fragment with a size of about 500 bp was obtained. The PCR product was recovered, connected into pBluescript IISK(+), and sequenced to identify the missing sequence by the dideoxy termination method. See attached figure 1 , attached figure 2 .
[0052] 2. Pseudorabies virus E A strain TK - / gE - / gI - Construction of mutant strains:
[0053] PrV TK linearized with EcoR I from plasmid pFBBS - / gE - / LacZ + Genomic DNA of mutant strains...
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