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C基因截短的HBV复制与包装
引用本文:韩聚强,胡大荣,熊锦华,胡学玲,范公忍,李娟,刘超英,邸雅南,吴忆贫. C基因截短的HBV复制与包装[J]. 中华实验和临床病毒学杂志, 2004, 18(1): 39-42
作者姓名:韩聚强  胡大荣  熊锦华  胡学玲  范公忍  李娟  刘超英  邸雅南  吴忆贫
作者单位:100700,北京军区总医院肝病研究所
基金项目:全军医药卫生科研基金资助项目 (0 1MA0 10 )
摘    要:
目的 探讨C基因截短型HBV变异体的复制与包装。方法 采用分子克隆、人工定点突变等技术构建C基因截短型HBV变异体质粒,用脂质体法转染HepG2细胞,提取细胞内及培养上清液中DNA分别进行Southem杂交,PCR及实时定量荧光PCR分析。结果 经DNA测序及酶切鉴定证实C基因截短型HBV质粒载体构建成功;C基因截短型HBV为复制缺损型,与辅助质粒共转染HepG2细胞,可在细胞内及培养上清液中检测到HBV各种DNA构型;DNA定量分析提示C基因截短型HBV的包装效率较野生型HBV提高3~40倍。结论 C基因截短型HBV变异体为复制缺损型,单独转染后不能在肝细胞内包装与复制,但在缺失包装信号ε的相应辅助病毒辅助下可有效复制并包装成子代病毒颗粒分泌到胞外,且包装效率大大提高。

关 键 词:C基因截短 HBV 病毒复制 病毒包装 乙型肝炎病毒 基因缺失 分子生物学
修稿时间:2003-10-08

Replication and encapsidation of HBV mutants with the truncated C gene
HAN Ju-qiang,HU Da-rong,XIONG Jin-hua,HU Xue-ling,FAN Gong-ren,LI Juan,LIU Chao-ying,DI Ya-nan,WU Yi-pin. Replication and encapsidation of HBV mutants with the truncated C gene[J]. Chinese journal of experimental and clinical virology, 2004, 18(1): 39-42
Authors:HAN Ju-qiang  HU Da-rong  XIONG Jin-hua  HU Xue-ling  FAN Gong-ren  LI Juan  LIU Chao-ying  DI Ya-nan  WU Yi-pin
Affiliation:Institute of Hepatology, Beijing Military General Hospital, Beijing 100700, China.
Abstract:
OBJECTIVE: To evaluate the replication and encapsidation of HBV mutants with the truncated C gene. METHODS: The HBV mutants with the truncated C gene were constructed by molecular cloning and PCR-based deletion in vitro. The replication and encapsidation of HBV mutants were investigated by Southern blotting, PCR and real-time fluorescence PCR respectively after transfecting the HBV mutants plasmid into HepG2 cells by using liposome. RESULTS: The C-truncated HBV mutant vectors were constructed successfully and confirmed exactly by clone sequencing and enzymes digestion. The C-truncated HBV mutants were replication defective, however, all types of HBV DNA could be detected positive in the cytoplasm and supernatant after co-transfecting the C-truncated HBV mutants plasmid and the helper constructs into HepG2 cells. The C-truncated HBV mutants were proved to produce 3-40 folds more progeny DNA than that of the wild-type HBV by DNA quantitative assay. CONCLUSION: The C-truncated HBV mutants are replication-deficient and could not replicate and encapsulate in the hepatocytes when transfected solely, however, the progeny HBV-variant viruses are encapsidated more effectively to secrete into supernatant when co-transfected with the helper construct which lacks part of 5 prime-proximal HBV RNA packaging signal Epsilon.
Keywords:Hepatitis B virus  Hepatitis B core antigens  DNA replication  Mutation (genetics)
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