Method for constructing and expressing multicopy gene co-expressing baculovirus exogenous protein
A baculovirus and exogenous protein technology, applied in the field of genetic engineering, can solve the problems of decreased expression efficiency of exogenous protein, no baculovirus expression system, etc., and achieve the effect of high-efficiency expression and increased expression
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[0041] A method for constructing and expressing a foreign protein of baculovirus co-expressed by using multiple copies of genes, comprising the following steps:
[0042] 1. PCR amplification of firefly luciferase gene:
[0043] Using the plasmid Pet28a-Fluc as a template, a pair of specific primers BSFlucF and XhoFlucR were designed, wherein the BSFlucF primer was added with BamHI and SmaI restriction sites, and the XhoFlucR primer was added with an XhoI restriction site. Utilize PCR method to amplify then and obtain Fluc gene fragment, gene sequence length is 1671bp (result see figure 1 ), after PCR amplification, the PCR product was sent to Beijing Huada Gene for sequencing verification.
[0044] 2. Construction of multi-copy exogenous gene transfer vector driven by p10 promoter:
[0045] The correctly sequenced Fluc gene fragment was digested by SmaI and XhoI and then ligated into the same restriction site of pFBDM-IG to obtain the vector pFBDM-p10F-IG; then pFBDM-p10F-IG...
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