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Transcription of the hepatitis B surface antigen gene in mouse cells transformed with cloned viral DNA.

机译:用克隆的病毒DNA转化的小鼠细胞中乙肝表面抗原基因的转录。

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摘要

Mouse L cells transformed with recombinant plasmids carrying hepatitis B virus (HBV) DNA fragments were used to study the transcription of the viral surface antigen gene (gene S). An HBV-specific, polyadenylated, 2.3-kilobase RNA was mapped on the HBV genome. This RNA hybridized with approximately 75% of the genome and excluded the region of the HBV core antigen gene (gene C). The 2.3-kilobase RNA species was present only in cell lines that produced hepatitis B surface antigen. An HBV-specific 2.3-kilobase RNA was also detected in human hepatoma cell line PLC/PRF/5 which produced hepatitis B surface antigen. A study of gene S expression in the transformed mouse L cells allowed us to localize the regions of initiation and termination of gene S transcription. Our results strongly suggest that the 2.3-kilobase RNA molecule is the mRNA of the major polypeptide of the envelope, which carries the viral surface antigen determinants.
机译:用携带乙型肝炎病毒(HBV)DNA片段的重组质粒转化的小鼠L细胞用于研究病毒表面抗原基因(基因S)的转录。将HBV特异性的聚腺苷酸2.3碱基碱基RNA定位在HBV基因组上。该RNA与大约75%的基因组杂交,并排除了HBV核心抗原基因(基因C)的区域。 2.3碱基碱基的RNA仅存在于产生乙型肝炎表面抗原的细胞系中。在产生乙型肝炎表面抗原的人肝癌细胞株PLC / PRF / 5中也检测到了HBV特异性2.3碱基碱基的RNA。对转化的小鼠L细胞中基因S表达的研究使我们能够定位基因S转录的起始和终止区域。我们的结果强烈表明,2.3碱基碱基的RNA分子是包膜的主要多肽的mRNA,其携带病毒表面抗原决定簇。

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