p10 genes of Bombyx mori nuclear polyhedrosis virus and Autographa californica multiple nuclear polyhedrosis virus.

Y Zhang, X Wu, Z Li
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Abstract

EcoR I-P fragment has been cloned from Autographa californica multiple nuclear polyhedrosis virus (AcMNPV) genomic DNA and used as a probe. 0.5-kb and 1.1-kb fragments including p10 gene from Bombyx mori nuclear polyhedrosis virus (BmNPV) have been hybridized. The p10 ORF was located in the EcoR I-R fragment. Initiation codon ATG of p10 from BmNPV has been mutated by PCR, and the ATG region became a Bgl II site. A novel transfer vector pBmAcPV-1 has been constructed using both the p10 5'-flanking region whose initiation codon ATG has been mutated with BmNPV and the p10 3'-flanking region of AcMNPV. The vector can recombine with not only AcMNPV DNA to express foreign gene in Sf cells, but also BmNPV DNA to express foreign gene in Bm cells. CAT gene was expressed at high level in Bm cells under the control of the mutated p10 promoter of BmNPV.

家蚕核型多角体病毒和加州签名虫核型多角体病毒的p10基因。
从加利福尼亚多核多角体病毒(AcMNPV)基因组DNA中克隆出EcoR I-P片段作为探针。对家蚕核型多角体病毒(BmNPV)含p10基因的0.5 kb和1.1 kb片段进行了杂交。p10 ORF位于EcoR I-R片段。BmNPV p10的起始密码子ATG通过PCR发生突变,ATG区域成为Bgl II位点。利用BmNPV突变起始密码子ATG的p10 5′-侧翼区和AcMNPV的p10 3′-侧翼区构建了新的转移载体pBmAcPV-1。该载体既可以与AcMNPV DNA重组,在Sf细胞中表达外源基因,也可以与BmNPV DNA重组,在Bm细胞中表达外源基因。在BmNPV突变的p10启动子的控制下,CAT基因在Bm细胞中高水平表达。
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