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在分离的线粒体和内质网膜中对两种 Tospovirus 的真实体外复制。

Authentic in vitro replication of two tombusviruses in isolated mitochondrial and endoplasmic reticulum membranes.

机构信息

Department of Plant Pathology, University of Kentucky, Lexington, Kentucky, USA.

出版信息

J Virol. 2012 Dec;86(23):12779-94. doi: 10.1128/JVI.00973-12. Epub 2012 Sep 12.

DOI:10.1128/JVI.00973-12
PMID:22973028
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3497632/
Abstract

Replication of plus-stranded RNA viruses takes place on membranous structures derived from various organelles in infected cells. Previous works with Tomato bushy stunt tombusvirus (TBSV) revealed the recruitment of either peroxisomal or endoplasmic reticulum (ER) membranes for replication. In case of Carnation Italian ringspot tombusvirus (CIRV), the mitochondrial membranes supported CIRV replication. In this study, we developed ER and mitochondrion-based in vitro tombusvirus replication assays. Using purified recombinant TBSV and CIRV replication proteins, we showed that TBSV could use the purified yeast ER and mitochondrial preparations for complete viral RNA replication, while CIRV preferentially replicated in the mitochondrial membranes. The viral RNA became partly RNase resistant after ∼40 to 60 min of incubation in the purified ER and mitochondrial preparations, suggesting that assembly of TBSV and CIRV replicases could take place in the purified ER and mitochondrial membranes in vitro. Using chimeric and heterologous combinations of replication proteins, we showed that multiple domains within the replication proteins are involved in determining the efficiency of tombusvirus replication in the two subcellular membranes. Altogether, we demonstrated that TBSV is less limited while CIRV is more restricted in utilizing various intracellular membranes for replication. Overall, the current work provides evidence that tombusvirus replication could occur in vitro in isolated subcellular membranes, suggesting that tombusviruses have the ability to utilize alternative organellar membranes during infection that could increase the chance of mixed virus replication and rapid evolution during coinfection.

摘要

正链 RNA 病毒的复制发生在感染细胞中各种细胞器衍生的膜结构上。以前对番茄丛矮病毒(TBSV)的研究表明,病毒复制可以招募过氧化物酶体或内质网(ER)膜。在香石竹意大利环斑病毒(CIRV)的情况下,线粒体膜支持 CIRV 的复制。在这项研究中,我们开发了基于 ER 和线粒体的体外 TBSV 复制测定法。使用纯化的重组 TBSV 和 CIRV 复制蛋白,我们表明 TBSV 可以使用纯化的酵母 ER 和线粒体制剂来完成病毒 RNA 的复制,而 CIRV 则优先在线粒体膜中复制。在纯化的 ER 和线粒体制剂中孵育约 40 至 60 分钟后,病毒 RNA 变得部分对核糖核酸酶具有抗性,这表明 TBSV 和 CIRV 复制酶的组装可以在体外的纯化 ER 和线粒体膜中进行。使用复制蛋白的嵌合和异源组合,我们表明复制蛋白中的多个结构域参与决定病毒在两种亚细胞膜中的复制效率。总之,我们证明 TBSV 的限制较少,而 CIRV 则在利用各种细胞内膜进行复制方面受到更多限制。总的来说,目前的工作提供了证据,表明在体外,TBSV 可以在分离的亚细胞膜中复制,这表明 TBSV 在感染过程中具有利用替代细胞器膜的能力,这可能增加混合病毒复制和共同感染期间快速进化的机会。

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2
A Co-Opted DEAD-Box RNA helicase enhances tombusvirus plus-strand synthesis.一种被篡夺的 DEAD-Box RNA 解旋酶增强了杆状病毒的正链合成。
PLoS Pathog. 2012 Feb;8(2):e1002537. doi: 10.1371/journal.ppat.1002537. Epub 2012 Feb 16.
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The TPR domain in the host Cyp40-like cyclophilin binds to the viral replication protein and inhibits the assembly of the tombusviral replicase.宿主 Cyp40 样亲环蛋白中的 TPR 结构域与病毒复制蛋白结合,抑制呼肠孤病毒复制酶的组装。
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An inhibitory function of WW domain-containing host proteins in RNA virus replication.宿主蛋白 WW 结构域在 RNA 病毒复制中的抑制功能。
Virology. 2012 May 10;426(2):106-19. doi: 10.1016/j.virol.2012.01.020. Epub 2012 Feb 16.
5
Synergistic roles of eukaryotic translation elongation factors 1Bγ and 1A in stimulation of tombusvirus minus-strand synthesis.真核翻译延伸因子 1Bγ 和 1A 在刺激番茄斑萎病毒负链合成中的协同作用。
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