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Continuous expression and replication of the hepatitis delta virus genome in Hep G2 hepatoblastoma cells transfected with cloned viral DNA.

机译:丙型肝炎三角洲病毒基因组在用克隆的病毒DNA转染的Hep G2肝母细胞瘤细胞中的连续表达和复制。

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摘要

To establish stable cell clones allowing continuous replication of hepatitis delta virus (HDV), Hep G2, a hepatoblastoma cell line containing no hepatitis B virus (HBV) DNA sequences, was transfected with a recombinant plasmid containing a tandem trimer of HDV cDNA (driven by the simian virus 40 late promoter) and a neomycin-resistance gene. After selection with the neomycin analogue G418, at least two of the resistant clones were shown to have intact delta antigen by specific immunoblotting, and the delta antigen was located in the cell nucleus by immunofluorescence. Transfected cloned viral DNAs were found to be integrated into cell chromosomes. Replication of the HDV genome was demonstrated by the presence of not only genomic and antigenomic HDV RNAs but also HDV RNAs in multimeric and circular forms. In addition, a 0.8-kilobase antigenomic RNA containing a poly(A) tail and encoding the delta-antigen open reading frame was documented. Continuous replication and transcription of the HDV genome was thus achieved in these transfected cell lines. The results confirmed that replication of HDV was unassisted by HBV. Stable passage of such cell lines strongly suggests that HDV lacks direct cytopathicity in hepatocytes. These clones should be useful in studying the details of the HDV life cycle and the relationship between HDV and its helper virus, HBV.
机译:为了建立稳定的细胞克隆以允许肝炎三角洲病毒(HDV)的连续复制,将Hep G2(一种不含乙肝病毒(HBV)DNA序列的肝母细胞瘤细胞系)用含有HDV cDNA串联三聚体的重组质粒转染(由猿猴病毒40个晚期启动子)和一个新霉素抗性基因。用新霉素类似物G418筛选后,至少有两个抗性克隆通过特异性免疫印迹显示出完整的delta抗原,并且通过免疫荧光将delta抗原定位在细胞核中。发现转染的克隆病毒DNA已整合到细胞染色体中。 HDV基因组的复制不仅通过基因组和反基因组HDV RNA的存在,而且还以多聚体和环状形式存在。另外,记录了一个0.8碱基碱基的反基因组RNA,它含有一个poly(A)尾巴并编码δ-抗原开放阅读框。因此,在这些转染的细胞系中实现了HDV基因组的连续复制和转录。结果证实,HBV不能促进HDV的复制。这些细胞系的稳定传代强烈提示HDV在肝细胞中缺乏直接的细胞病变。这些克隆应有助于研究HDV生命周期的细节以及HDV及其辅助病毒HBV之间的关系。

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