Construction and Application of Recombinant Turkey Herpes Virus Expressing Chicken Newcastle Disease Virus f Gene
A technology of turkey herpes virus and chicken Newcastle disease virus, applied in the field of animal virology, can solve the problems of short vaccine immune protection period, increased susceptibility to secondary bacterial infection, and strong NDV infection
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Embodiment 1
[0038] ——Construction of rHVT-F recombinant virus
[0039] 1. Preparation of an expression cassette (see sequence 1 for the sequence) containing the F gene of chicken Newcastle disease virus
[0040] Design and amplify NDV F gene primer NDV-F-F / R (SEQ ID NO:2 / SEQ ID NO:3). Using the extracted NDV RNA as a template, the NDV F gene fragment was amplified by RT-PCR, digested with Nhe I and Xba I, and cloned into the eukaryotic expression vector pcDNA3.1, and the obtained positive plasmid was named pcDNA3.1 / NDV-F. According to Lipofectamine2000 (Thermo Fisher Scientific) transfection method, the recombinant plasmid pcDNA3.1 / NDV-F was transfected into CEF cells, and the expression of recombinant plasmid F protein was identified with the monoclonal antibody of NDV F protein as the primary antibody.
[0041] Table 1 Primers used to construct recombinant plasmids.
[0042]
[0043] 2. Construction of recombinant plasmids containing homology arms and expression cassettes
[004...
Embodiment 2
[0052] ——Study on the stability of rHVT-F recombinant virus in cells
[0053] The purified recombinant virus HVT-F1 was continuously passaged on CEF cells, and the 10th, 20th, and 30th generation recombinant viruses were selected for indirect immunofluorescence identification to detect the expression of NDV F gene. Extract different generations of viral DNA, use PCR to amplify the chimeric region of the foreign gene of the recombinant virus, and perform sequencing verification. Using different generations of DNA as templates, specific fragments of the chimeric region of the NDV F gene expression cassette with a length of about 600 bp can be amplified. The results showed that the NDV F gene could stably exist and express in the recombinant virus HVT-F1. The primers used are:
[0054] qianhe-F:5'-GCACATCTGC TCTCATTAC C-3'21 (SEQ ID NO: 14)
[0055] qianhe-R:5'-GTTTCAAATT TTCACGATTC C-3'21 (SEQ ID NO: 15)
Embodiment 3
[0057] ——Evaluation of immune efficacy of recombinant virus rHVT-F in SPF chickens
[0058] Sixty 1-day-old SPF chickens were randomly divided into 3 groups. The first group was vaccinated with rHVT-F, and the immunization dose was 4000PFU / bird. The second group is a non-immune challenge group, and the third group is a blank control (non-immune non-challenge) group. At the age of 21 days, the virulent Beijing strain of NDV was challenged, and the protection rate of rHVT-F reached 90% after 14 days of observation (see Table 2).
[0059] Table 2 The immune protection effect of rHVT-F on SPF chickens
[0060] group challenge strain Deaths (rate) Protection rate (%) rHVT-F vaccine immunization group NDV (Beijing Branch) 2 / 20(10%) 90 Challenge control group- NDV (Beijing Branch) 20 / 20(0%) 0 Blank control group- - 0 / 20(0%) -
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