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丁型肝炎病毒在自然混合基因型感染及转染培养细胞中的RNA重组

RNA recombination of hepatitis delta virus in natural mixed-genotype infection and transfected cultured cells.

作者信息

Wang Tzu-Chi, Chao Mei

机构信息

Department of Microbiology and Immunology, College of Medicine, Chang Gung University, 259, Wen-Hwa 1st Rd., Kwei-Shan, Tao-yang 333, Taiwan.

出版信息

J Virol. 2005 Feb;79(4):2221-9. doi: 10.1128/JVI.79.4.2221-2229.2005.

Abstract

Most RNA viruses encode their own RNA polymerases for genome replication, and increasing numbers of them appear to be capable of undergoing RNA recombination. Here, we provide the first report of intergenotypic recombination in hepatitis delta virus (HDV), the only animal RNA virus that requires host RNA polymerase(s) for viral replication. In vivo, we analyzed RNA species derived from the serum of a patient with mixed genotype I and genotype IIb HDV infection by using multiple restriction fragment length polymorphism (RFLP) assays and sequence analysis of cloned reverse transcription (RT)-PCR products. Six HDV recombinants were isolated from 101 tested clones, and HDV recombination in this patient was further confirmed by RT-PCR with genotype-specific primer pairs. Analysis of the recombination junctions suggested that the HDV genome rearrangement occurred through faithful homologous recombination. We then used an RNA cotransfection cell culture system to investigate HDV RNA recombination in vitro. We found that HDV recombinants could indeed be detected in the transfected cells; some of these possessed recombination junctions identical to those identified in vivo. Furthermore, using a PCR-independent RNase protection assay, we were able to readily identify the recombined HDV RNA species in cultured cells. Taken together, our results demonstrate that HDV RNA recombination occurs in both natural HDV infections and cultured cells, thereby presenting a novel mechanism for HDV evolution.

摘要

大多数RNA病毒编码自身的RNA聚合酶用于基因组复制,并且越来越多的RNA病毒似乎能够进行RNA重组。在此,我们首次报道了丁型肝炎病毒(HDV)的基因型间重组,HDV是唯一一种需要宿主RNA聚合酶进行病毒复制的动物RNA病毒。在体内,我们通过使用多种限制性片段长度多态性(RFLP)分析以及对克隆的逆转录(RT)-PCR产物进行序列分析,来分析一名同时感染I型和IIb型HDV混合基因型患者血清中的RNA种类。从101个测试克隆中分离出6个HDV重组体,并且通过使用基因型特异性引物对进行RT-PCR进一步证实了该患者体内的HDV重组。对重组连接点的分析表明,HDV基因组重排是通过忠实的同源重组发生的。然后,我们使用RNA共转染细胞培养系统在体外研究HDV RNA重组。我们发现,在转染细胞中确实能够检测到HDV重组体;其中一些重组体具有与在体内鉴定出的相同的重组连接点。此外,使用一种不依赖PCR的核糖核酸酶保护试验,我们能够轻松地在培养细胞中鉴定出重组的HDV RNA种类。综上所述,我们的结果表明,HDV RNA重组在自然HDV感染和培养细胞中均会发生,从而为HDV进化提供了一种新机制。

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