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本文引用的文献

1
Rotavirus open cores catalyze 5'-capping and methylation of exogenous RNA: evidence that VP3 is a methyltransferase.轮状病毒开放核心催化外源RNA的5'-加帽和甲基化:VP3是一种甲基转移酶的证据。
Virology. 1999 Dec 5;265(1):120-30. doi: 10.1006/viro.1999.0029.
2
Multimers formed by the rotavirus nonstructural protein NSP2 bind to RNA and have nucleoside triphosphatase activity.由轮状病毒非结构蛋白NSP2形成的多聚体与RNA结合并具有核苷三磷酸酶活性。
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3
Open reading frame in rotavirus mRNA specifically promotes synthesis of double-stranded RNA: template size also affects replication efficiency.轮状病毒信使核糖核酸中的开放阅读框特异性地促进双链核糖核酸的合成:模板大小也影响复制效率。
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RNA-binding and capping activities of proteins in rotavirus open cores.轮状病毒开放核心中蛋白质的RNA结合与加帽活性
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Rotavirus RNA replication requires a single-stranded 3' end for efficient minus-strand synthesis.轮状病毒RNA复制需要一个单链3'末端以高效合成负链。
J Virol. 1998 Sep;72(9):7387-96. doi: 10.1128/JVI.72.9.7387-7396.1998.
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Rotavirus RNA polymerase requires the core shell protein to synthesize the double-stranded RNA genome.轮状病毒RNA聚合酶需要核心壳蛋白来合成双链RNA基因组。
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Three-dimensional structural analysis of recombinant rotavirus-like particles with intact and amino-terminal-deleted VP2: implications for the architecture of the VP2 capsid layer.具有完整和氨基末端缺失的VP2的重组轮状病毒样颗粒的三维结构分析:对VP2衣壳层结构的影响
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Comparison of the replication of positive-stranded RNA viruses of plants and animals.植物和动物正链RNA病毒复制的比较。
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Rotavirus VP1 alone specifically binds to the 3' end of viral mRNA, but the interaction is not sufficient to initiate minus-strand synthesis.单独的轮状病毒VP1特异性结合病毒mRNA的3'末端,但这种相互作用不足以启动负链合成。
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10
The 3'-terminal consensus sequence of rotavirus mRNA is the minimal promoter of negative-strand RNA synthesis.轮状病毒mRNA的3'末端共有序列是负链RNA合成的最小启动子。
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轮状病毒RNA聚合酶在无细胞系统中从头合成负链RNA涉及一种新的起始机制。

De novo synthesis of minus strand RNA by the rotavirus RNA polymerase in a cell-free system involves a novel mechanism of initiation.

作者信息

Chen D, Patton J T

机构信息

Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

RNA. 2000 Oct;6(10):1455-67. doi: 10.1017/s1355838200001187.

DOI:10.1017/s1355838200001187
PMID:11073221
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1370016/
Abstract

The replicase activity of rotavirus open cores has been used to study the synthesis of (-) strand RNA from viral (+) strand RNA in a cell-free replication system. The last 7 nt of the (+) strand RNA, 5'-UGUGACC-3', are highly conserved and are necessary for efficient (-) strand synthesis in vitro. Characterization of the cell-free replication system revealed that the addition of NaCl inhibited (-) strand synthesis. By preincubating open cores with (+) strand RNA and ATP, CTP, and GTP prior to the addition of NaCl and UTP, the salt-sensitive step was overcome. Thus, (-) strand initiation, but not elongation, was a salt-sensitive process in the cell-free system. Further analysis of the requirements for initiation showed that preincubating open cores and the (+) strand RNA with GTP or UTP, but not with ATP or CTP, allowed (-) strand synthesis to occur in the presence of NaCl. Mutagenesis suggested that in the presence of GTP, (-) strand synthesis initiated at the 3'-terminal C residue of the (+) strand template, whereas in the absence of GTP, an aberrant initiation event occurred at the third residue upstream from the 3' end of the (+) strand RNA. During preincubation with GTP, formation of the dinucleotides pGpG and ppGpG was detected; however, no such products were made during preincubation with ATP, CTP, or UTP. Replication assays showed that pGpG, but not GpG, pApG, or ApG, served as a specific primer for (-) strand synthesis and that the synthesis of pGpG may occur by a template-independent process. From these data, we conclude that initiation of rotavirus (-) strand synthesis involves the formation of a ternary complex consisting of the viral RNA-dependent RNA polymerase, viral (+) strand RNA, and possibly a 5'-phosphorylated dinucleotide, that is, pGpG or ppGpG.

摘要

轮状病毒开放核心的复制酶活性已被用于在无细胞复制系统中研究从病毒(+)链RNA合成(-)链RNA。(+)链RNA的最后7个核苷酸,5'-UGUGACC-3',高度保守,是体外高效合成(-)链所必需的。对无细胞复制系统的特性分析表明,添加NaCl会抑制(-)链合成。通过在添加NaCl和UTP之前,将开放核心与(+)链RNA以及ATP、CTP和GTP预孵育,可以克服盐敏感步骤。因此,在无细胞系统中,(-)链起始而非延伸是一个盐敏感过程。对起始需求的进一步分析表明,将开放核心和(+)链RNA与GTP或UTP而非ATP或CTP预孵育,可使(-)链合成在有NaCl存在的情况下发生。诱变表明,在有GTP存在时,(-)链合成在(+)链模板的3'-末端C残基处起始,而在无GTP时,异常起始事件发生在(+)链RNA 3'端上游的第三个残基处。在与GTP预孵育期间,检测到二核苷酸pGpG和ppGpG的形成;然而,在与ATP、CTP或UTP预孵育期间未产生此类产物。复制试验表明,pGpG而非GpG、pApG或ApG作为(-)链合成的特异性引物,并且pGpG的合成可能通过模板非依赖过程发生。从这些数据中,我们得出结论,轮状病毒(-)链合成的起始涉及由病毒RNA依赖性RNA聚合酶、病毒(+)链RNA以及可能的5'-磷酸化二核苷酸(即pGpG或ppGpG)组成的三元复合物的形成。