A kind of recombinant Newcastle disease virus expressing goose parvovirus vp3 gene and its construction method
A technology of Newcastle disease virus and goose parvovirus, applied in the field of recombinant Newcastle disease virus expressing goose parvovirus VP3 gene and its construction, can solve the problems of goose farming hazards, potential infection and detoxification, complex preparation process, etc.
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Embodiment 1
[0033] Embodiment 1 Construction of Newcastle disease virus reverse genetics operating system
[0034] 1 Materials and methods
[0035] 1.1 Materials
[0036] Newcastle disease virus NA-1 strain (GenBank: DQ659677.1); BHK-21 cells (ATCC No.CCL-10), the culture medium is DMEM containing 10% fetal bovine serum; plasmids pCI (Promega) and pBluescript II KS+ ( Clontech); Phusion DNA polymerase, T4 DNA ligase and other restriction endonucleases were purchased from NEB Company; competent cells were purchased from TaKaRa Company; gel recovery kit and plasmid extraction kit were purchased from OMEGA Company; RNA extraction TRIzol, mouse-derived reverse transcriptase MLV, calcium phosphate transfection kit, RPMI1640 culture medium were purchased from Invitrogen; chicken anti-NDV whole virus hyperimmune serum; fluorescein (FITC)-labeled goat anti-chicken secondary antibody was purchased from Sigma; The fluorescent microscope was BX51FL; Olympus was purchased from Olympus Company, cell...
Embodiment 2
[0059] Example 2 Mutation of F cleavage site and construction of full-length cDNA clone expressing goose parvovirus (GPV) VP3 gene
[0060] 1 Materials and methods
[0061] 1.1 Materials
[0062] With embodiment 1.
[0063] 1.2 Construction of full-length plasmid expressing VP3 gene
[0064] On the basis of the above-mentioned NDV genome full-length cDNA clone pCI-NA-1, design mutation primers as follows:
[0065]
[0066] Note: The italics in the primer Fmut-R are the cleavage site sequence of F protein, and the mutation site is underlined.
[0067]The PCR method is used to mutate the 4883-4900nt of the full-length cDNA clone, so that the encoded amino acid is mutated from the highly toxic characteristic sequence RRQKRF to the weakly toxic characteristic sequence GRQGRL. The open reading frame sequence of GPV GD-01 strain VP3 (GenBank Accession No.DQ665790) was obtained from GenBank, and primers were designed, and the upstream primer was introduced into the PmeI restri...
Embodiment 3
[0086] Embodiment 3 Chicken embryo growth characteristics comparison
[0087] 1 Materials and methods
[0088] 1.1 Materials
[0089] SPF chicken embryos were purchased from Beijing Merial, 96-well hemagglutination plate, fresh chicken blood, phosphate buffered saline (PBS), incubator, etc.
[0090] 1.2 Method
[0091] In order to determine the growth characteristics of rescued recombinant virus rNA-1, rNA-VP3 and maternal wild-type NA-1 chick embryo, the recombinant virus rNA-1 and rNA-VP3 F3 generation allantoic fluid and wild-type rNA-1 allantoic fluid Diluted in PBS to 1×10 4 EID 50 Inoculate the allantoic cavity of chicken embryos with SPF. Samples were taken at 24 hours, 48 hours, 72 hours and 96 hours after inoculation, 6 embryos were randomly selected at each time point, the allantoic fluid was collected, and the EID was measured after mixing 50 .
[0092] 2 results
[0093] In order to identify the growth characteristics of the rescue mutant strain and the w...
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