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HIV-1 mRNA的转录后m(6)A编辑增强病毒基因表达。

Posttranscriptional m(6)A Editing of HIV-1 mRNAs Enhances Viral Gene Expression.

作者信息

Kennedy Edward M, Bogerd Hal P, Kornepati Anand V R, Kang Dong, Ghoshal Delta, Marshall Joy B, Poling Brigid C, Tsai Kevin, Gokhale Nandan S, Horner Stacy M, Cullen Bryan R

机构信息

Department of Molecular Genetics and Microbiology, Duke University Medical Center, Durham, NC 27710, USA.

Department of Molecular Genetics and Microbiology, Duke University Medical Center, Durham, NC 27710, USA; Department of Medicine, Duke University Medical Center, Durham, NC 27710, USA.

出版信息

Cell Host Microbe. 2016 May 11;19(5):675-85. doi: 10.1016/j.chom.2016.04.002. Epub 2016 Apr 21.

DOI:10.1016/j.chom.2016.04.002
PMID:27117054
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4867121/
Abstract

Covalent addition of a methyl group to adenosine N(6) (m(6)A) is an evolutionarily conserved and common RNA modification that is thought to modulate several aspects of RNA metabolism. While the presence of multiple m(6)A editing sites on diverse viral RNAs was reported starting almost 40 years ago, how m(6)A editing affects virus replication has remained unclear. Here, we used photo-crosslinking-assisted m(6)A sequencing techniques to precisely map several m(6)A editing sites on the HIV-1 genome and report that they cluster in the HIV-1 3' untranslated region (3' UTR). Viral 3' UTR m(6)A sites or analogous cellular m(6)A sites strongly enhanced mRNA expression in cis by recruiting the cellular YTHDF m(6)A "reader" proteins. Reducing YTHDF expression inhibited, while YTHDF overexpression enhanced, HIV-1 protein and RNA expression, and virus replication in CD4+ T cells. These data identify m(6)A editing and the resultant recruitment of YTHDF proteins as major positive regulators of HIV-1 mRNA expression.

摘要

将甲基共价添加到腺苷的N(6)位(m(6)A)是一种进化上保守且常见的RNA修饰,被认为可调节RNA代谢的多个方面。虽然近40年前就已报道多种病毒RNA上存在多个m(6)A编辑位点,但m(6)A编辑如何影响病毒复制仍不清楚。在此,我们使用光交联辅助的m(6)A测序技术精确绘制了HIV-1基因组上的多个m(6)A编辑位点,并报告它们聚集在HIV-1 3'非翻译区(3'UTR)。病毒3'UTR的m(6)A位点或类似的细胞m(6)A位点通过招募细胞YTHDF m(6)A“读取器”蛋白在顺式作用中强烈增强mRNA表达。降低YTHDF表达会抑制HIV-1蛋白和RNA表达以及CD4+ T细胞中的病毒复制,而YTHDF过表达则会增强这些过程。这些数据表明m(6)A编辑以及由此导致的YTHDF蛋白募集是HIV-1 mRNA表达的主要正调控因子。

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