一种新型家蚕核多角体病毒Bac to Bac系统的构建

用家蚕核型多角体病毒的全基因组ＤＮＡ与Ａｃ－ＢａｃｉｍｉｄＤＮＡ共转染家蚕ＢｍＮ细胞，构建转座一穿梭载体Ｂｍ－Ｂａｃｍｉｄ。另一供体质粒以转座方式将乙肝病毒ｅ抗的基因ＨＢｅＡｇ整合到Ｂｍ－Ｂａｃｍｉｄ的ａｔｔＴｎ７位点上成为重组ｒＢｍＨＢｅ。结果表明Ｂｍ－Ｂａｃｍｉｄ既能在大肠杆菌中以质粒的形式复制，又能在家蚕ＢｍＮ细胞和草地夜蛾Ｓｆ９细胞中复制，形成感染性病毒粒子。Ｓｏｕｔｈｅｒｎｂｌｏｔｔｉｎ

CONSTRUCTION OF A NOVEL Bm NPV Bac to Bac SYSTEM

A Bi-Shuttle vector Bm-Bacmid was constructed by co-infecting Bm N cells with wild type genomic DNA from BmNPV and Ac-Bacmid DNA. It could not only replicate in E. coli cells as a large plasmid and but also remain infectious when induced into Bm N or Sf9 cells. Recombinant virus rBmHBe was obtained after transposition of a donor plasmid carrying Hepatitis Be antigen gene (HBeAg) into att Tn7, and was demonstrated by Southern blotting. SDS-PAGE analysis showed that HBeAg gene were highly expressed in Bm N cells. By ELISA testing, the highest antigenecity titer of HBeAg protein in cell cultural medium was up to a dilution of 1:32,000. Although HBeAg protein also presented in the Bm N cells the titer was only 1:2000. The HBcAg protein was much fewer than HBeAg (< 1:160) whatever in culture medium and in cells. The results showed that Bm N cells was able to recognize the signal peptide sequence and cut it correctly for HBeAg protein's excreting production.