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作 者:唐红[1] 林勇[1] 王锦蓉[1] 刘丽[1] 赵连三[1] 穆仁懋[1] 雷秉钧[1]
机构地区:[1]华西医科大学病毒性肝炎研究室
出 处:《中华传染病杂志》1997年第1期28-31,共4页Chinese Journal of Infectious Diseases
基 金:国家自然科学青年基金;纽约中华医学基金
摘 要:为建立HDV的体外细胞培养系统,采用体外细胞转染技术,用含全基因HDVcDNA三聚体的重组质粒pSVLD3转染HBV的体外细胞培养株(2.2.15细胞株)。结果在转染后3天的转染细胞内和培养上清中检出了1.7KbHDVRNA和24000、27000HDAg。初步结果提示:该转染细胞培养上清中有HDV病毒的排泌,从而建立了HDV的体外短期细胞培养系统。In order to establish the HDV cell culture system, by using in vitro transfection technique, the in vitro cell line of HBV (2.2.15 cell line) was transfected by a recombinant plasmid containing full length trimer of HDV cDNA (pSVL D3). HDV RNA was detected by spot and Northern blot hybridization using Dig HDV cDNA probe, and HDAg was detected by immunobloting method. The results showed that three days after transfection, 1.7Kb HDV RNA and 24000, 27000 HDAg were detected in the transfected cells and in its culture medium. The primary results demonstrated that hepatitis D virus was assemblied and released in the transfected cell culture medium, so an in vitro transient cell culture system of HDV had been established.
分 类 号:R373.21[医药卫生—病原生物学]
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