Determination of RNA structural diversity and its role in HIV-1 RNA splicing

被引:0
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作者
Phillip J. Tomezsko
Vincent D. A. Corbin
Paromita Gupta
Harish Swaminathan
Margalit Glasgow
Sitara Persad
Matthew D. Edwards
Lachlan Mcintosh
Anthony T. Papenfuss
Ann Emery
Ronald Swanstrom
Trinity Zang
Tammy C. T. Lan
Paul Bieniasz
Daniel R. Kuritzkes
Athe Tsibris
Silvi Rouskin
机构
[1] Whitehead Institute for Biomedical Research,Program in Virology
[2] Harvard Medical School,Bioinformatics Division
[3] Brigham and Women’s Hospital,Department of Medical Biology
[4] Walter and Eliza Hall Institute,Computer Science and Artificial Intelligence Laboratory
[5] The University of Melbourne,Department of Mathematics and Statistics
[6] Massachusetts Institute of Technology,Sir Peter MacCallum Department of Oncology
[7] Massachusetts Institute of Technology,Curriculum in Genetics and Molecular Biology
[8] Peter MacCallum Cancer Centre,Lineberger Comprehensive Cancer Center
[9] University of Melbourne,Department of Microbiology and Immunology
[10] The University of Melbourne,Department of Biochemistry and Biophysics
[11] University of North Carolina at Chapel Hill,Laboratory of Retrovirology
[12] University of North Carolina at Chapel Hill,Howard Hughes Medical Institute
[13] University of North Carolina at Chapel Hill,Department of Medicine
[14] University of North Carolina at Chapel Hill,undefined
[15] The Rockefeller University,undefined
[16] The Rockefeller University,undefined
[17] Harvard Medical School,undefined
来源
Nature | 2020年 / 582卷
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摘要
Human immunodeficiency virus 1 (HIV-1) is a retrovirus with a ten-kilobase single-stranded RNA genome. HIV-1 must express all of its gene products from a single primary transcript, which undergoes alternative splicing to produce diverse protein products that include structural proteins and regulatory factors1,2. Despite the critical role of alternative splicing, the mechanisms that drive the choice of splice site are poorly understood. Synonymous RNA mutations that lead to severe defects in splicing and viral replication indicate the presence of unknown cis-regulatory elements3. Here we use dimethyl sulfate mutational profiling with sequencing (DMS-MaPseq) to investigate the structure of HIV-1 RNA in cells, and develop an algorithm that we name ‘detection of RNA folding ensembles using expectation–maximization’ (DREEM), which reveals the alternative conformations that are assumed by the same RNA sequence. Contrary to previous models that have analysed population averages4, our results reveal heterogeneous regions of RNA structure across the entire HIV-1 genome. In addition to confirming that in vitro characterized5 alternative structures for the HIV-1 Rev responsive element also exist in cells, we discover alternative conformations at critical splice sites that influence the ratio of transcript isoforms. Our simultaneous measurement of splicing and intracellular RNA structure provides evidence for the long-standing hypothesis6–8 that heterogeneity in RNA conformation regulates splice-site use and viral gene expression.
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页码:438 / 442
页数:4
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