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诺如病毒3D聚合酶引发的蛋白质引发和RNA合成的从头起始

Protein-primed and de novo initiation of RNA synthesis by norovirus 3Dpol.

作者信息

Rohayem Jacques, Robel Ivonne, Jäger Katrin, Scheffler Ulrike, Rudolph Wolfram

机构信息

Institut für Virologie, The Calicilab, Fiedlerstrasse 42, D-01307 Dresden, Germany.

出版信息

J Virol. 2006 Jul;80(14):7060-9. doi: 10.1128/JVI.02195-05.

Abstract

Noroviruses (Caliciviridae) are RNA viruses with a single-stranded, positive-oriented polyadenylated genome. To date, little is known about the replication strategy of norovirus, a so-far noncultivable virus. We have examined the initiation of replication of the norovirus genome in vitro, using the active norovirus RNA-dependent RNA polymerase (3D(pol)), homopolymeric templates, and synthetic subgenomic or antisubgenomic RNA. Initiation of RNA synthesis on homopolymeric templates as well as replication of subgenomic polyadenylated RNA was strictly primer dependent. In this context and as observed for other enteric RNA viruses, i.e., poliovirus, a protein-primed initiation of RNA synthesis after elongation of the VPg by norovirus 3D(pol) was postulated. To address this question, norovirus VPg was expressed in Escherichia coli and purified. Incubation of VPg with norovirus 3D(pol) generated VPg-poly(U), which primed the replication of subgenomic polyadenylated RNA. In contrast, replication of antisubgenomic RNA was not primer dependent, nor did it depend on a leader sequence, as evidenced by deletion analysis of the 3' termini of subgenomic and antisubgenomic RNA. On nonpolyadenylated RNA, i.e., antisubgenomic RNA, norovirus 3D(pol) initiated RNA synthesis de novo and terminated RNA synthesis by a poly(C) stretch. Interestingly, on poly(C) RNA templates, norovirus 3D(pol) initiated RNA synthesis de novo in the presence of high concentrations of GTP. We propose a novel model for initiation of replication of the norovirus genome by 3D(pol), with a VPg-protein-primed initiation of replication of polyadenylated genomic RNA and a de novo initiation of replication of antigenomic RNA.

摘要

诺如病毒(杯状病毒科)是一种具有单链、正向多聚腺苷酸化基因组的RNA病毒。迄今为止,对于诺如病毒(一种目前尚无法培养的病毒)的复制策略知之甚少。我们使用活性诺如病毒RNA依赖性RNA聚合酶(3D(pol))、同聚物模板以及合成的亚基因组或反亚基因组RNA,在体外研究了诺如病毒基因组的复制起始。在同聚物模板上的RNA合成起始以及亚基因组多聚腺苷酸化RNA的复制严格依赖引物。在这种情况下,正如对其他肠道RNA病毒(即脊髓灰质炎病毒)所观察到的那样,推测诺如病毒3D(pol)在VPg延伸后会进行蛋白引发的RNA合成起始。为了解决这个问题,诺如病毒VPg在大肠杆菌中表达并纯化。将VPg与诺如病毒3D(pol)一起温育会产生VPg-聚(U),它可引发亚基因组多聚腺苷酸化RNA的复制。相比之下,反亚基因组RNA的复制不依赖引物,也不依赖前导序列,亚基因组和反亚基因组RNA 3'末端的缺失分析证明了这一点。在非多聚腺苷酸化RNA(即反亚基因组RNA)上,诺如病毒3D(pol)从头起始RNA合成,并通过一个聚(C)序列终止RNA合成。有趣的是,在聚(C)RNA模板上,诺如病毒3D(pol)在高浓度GTP存在的情况下从头起始RNA合成。我们提出了一种由3D(pol)引发诺如病毒基因组复制起始的新模型,即多聚腺苷酸化基因组RNA的复制由VPg蛋白引发起始,而反基因组RNA的复制则从头起始。

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