Engineered bombyx mori baculovirus vector and method of increasing the NS1 expression amount by utilization of the vector
A technology of silkworm baculovirus and expression quantity, applied in the field of genetic engineering, can solve the problems of high production cost, difficulty in rapid determination, lack of fluorescent signal in BEVS system, etc.
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Embodiment 1
[0029] Example 1. Construction of recombinant plasmid pUC119-US-Cm-egfp-DS
[0030] Four pairs of specific primers were designed using Primer Premier5.0 software. First, through US-F: 5'-GC AAGCTT CGTA TGCGTTTTGCTCGT-3'(HindⅢ) (SEQ ID NO.1) and US-R:5'-AA CTGCAG Two specific primers CGCGCCAAGTTGG AACT-3'(PstI)(SEQ ID NO.2) specifically amplify a 538bp specific US fragment from the silkworm baculovirus genome, and the purified DNA fragment is purified with the same double enzyme The cut pUC119 plasmid was connected to obtain the recombinant plasmid pUC119-US; through Cm-F:5'-AA CTGCAG CTTCGAATAAATACCTGTGA-3'(PstI) (SEQ ID NO.3) and Cm-R:5'-AA TCTAGA AACCAGCAATAGACATAAGC-3' (XbaI) (SEQ ID NO.4) primer pair, amplify the Cm gene expression cassette that is 1039bp in length from the pUC18-Cm plasmid, the Cm gene expression cassette after PstI and XbaI double enzyme digestion is the same as The double digested pUC119-US was ligated to obtain the recombinant plasmid pUC119-US...
Embodiment 2
[0031] Example 2. Identification of recombinant plasmid pUC119-US-Cm-egfp-DS
[0032] Due to complex restriction sites in the recombinant plasmid, the recombinant plasmid was identified by multiple rounds of PCR (such as figure 2shown). Lane 1: US-F / US-R primer pair amplifies US, the product length is 551bp; Swimming lane 2: Cm-F / Cm-R primer pair amplifies the Cm gene expression cassette, the product length is 1079bp; lane3: egfp-F / egfp-R primer pair amplifies the egfp expression cassette, the product length is 1544bp; lane 4: DS-F / DS-R primer pair amplifies the DS fragment, the product length is 514bp; lane 5: US-F / Cm-R primer For amplifying US-Cm, the product length is 1630bp; lane 6: US-F / egfp-R primer pair amplifies US-Cm-egfp, and the product length is 3174bp; lane7: US-F / DS-R primer pair amplifies US-Cm-egfp-DS, the product length is 3688bp; lane 8: Cm-F / egfp-R primer pair amplifies Cm-egfp, the product length is 2623bp; lane9: Cm-F / DS-R primer pair amplifies Cm -eg...
Embodiment 3
[0034] Embodiment 3. Integrating the cascaded Cm and egfp gene expression cassettes into the silkworm Bm-Bacmid
[0035] Perform PCR amplification on the identified recombinant plasmid pUC119-US-Cm-egfp-DS by US-F / DS-R to obtain the quadruple target fragment US-Cm-egfp-DS, take 5ng of the purified amplification product, and transform In Escherichia coli DH10B competent cells captured with the silkworm shuttle vector Bm-Bacmid, in theory, under the action of homologous recombinase, US-Cm-egfp-DS and the Chitinase and Cystein Protease genes in the silkworm shuttle vector Bm-Bacmid were generated Double crossover, Chitinase and Cystein Protease gene deletion type Bm-Bacmid was obtained, meanwhile, a tandem Cm-egfp gene expression cassette was inserted at the missing Chitinase and Cystein Protease gene locus. by adding K + A + cm + (50 μg / ml kanamycin, 50 μg / ml ampicillin, 25 μg / ml chloramphenicol) three kinds of antibiotic plates were used for preliminary screening of recombin...
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