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作 者:李迎秋[1] 龙綮新[1] 徐帆[1] 江立敏 庞义[1]
出 处:《病毒学报》1997年第4期325-331,共7页Chinese Journal of Virology
摘 要:通过PCR获得长度为640bp的HBVpreC/C基因片段,将其克隆入转移载体质粒pSXIVVI+X3/4,构建出重组质粒pSXIVVI+X3/4-pC/C。利用共转染的方法,构建出既能形成多角体又能表达preC/C基因的重组毒株TnNPV-pC/C-OCC+。该重组毒株中preC/C基因受到串联的双启动子-合成启动子和含HindⅢ接头的XIV启动子的双重调控。对感染重组毒株的草地夜蛾(Spodopterafrugiperda,Sf)细胞及其培养上清分别进行HBeAg、HBcAg固相放射免疫检测,发现受感染细胞及其培养上清均呈HBeAg阳性,HBcAg阴性;进一步做Western分析表明,受感染细胞总蛋白中26kD及培养上清15kD处,呈现与HBeAg单克隆抗体特异性反应条带。结果表明,克隆的乙肝病毒preC/C基因在杆状病毒载体系统中得到正确表达和加工,加工产物能够有效分泌。The PCR-amplified HBV preC/C gene(640bp) was inserted into the transfer vector pSXIVVI +X3/4, the resultant pSXIVVI +X3/4-pC/C cotransfected Spodoptera frugiperda (Sf) cells with the parental virus(TnNPV-SVI --G) DNA to roduce the recombinant virus TnNPV-pC/C-OCC +, in which the preC/C gene was driven by the synthetic and XIV promoters. When HBeAg and HBcAg were detected by solid-phase radioimmunoassay, the cell lysates and the media from TnNPV-pC/C-OCC +-infected Sf cells were HBeAg positive and HBcAg negative. The Western blot analysis showed that the preC/C gene product, 26kD protein, was processed and secreted as 15kD protein. These results demonstrated that the preC/C gene product can be processed and secreted HBeAg efficiently in baculovirus vector system.
分 类 号:R373.21[医药卫生—病原生物学]
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