SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness

Converting single-stranded viral RNA into double stranded DNA for integration is an essential step in HIV-1 replication. Initial polymerization of minus-strand DNA is primed from a host derived tRNA, whereas subsequent plus-strand synthesis requires viral primers derived from the 3′ and central poly...

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Autores principales: Rausch, Jason W., Tian, Meijuan, Li, Yuejin, Angelova, Lora, Bagaya, Bernard S., Krebs, Kendall C., Qian, Feng, Zhu, Chuanwu, Arts, Eric J., Le Grice, Stuart F. J., Gao, Yong
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4393142/
https://www.ncbi.nlm.nih.gov/pubmed/25860884
http://dx.doi.org/10.1371/journal.pone.0122953
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author Rausch, Jason W.
Tian, Meijuan
Li, Yuejin
Angelova, Lora
Bagaya, Bernard S.
Krebs, Kendall C.
Qian, Feng
Zhu, Chuanwu
Arts, Eric J.
Le Grice, Stuart F. J.
Gao, Yong
author_facet Rausch, Jason W.
Tian, Meijuan
Li, Yuejin
Angelova, Lora
Bagaya, Bernard S.
Krebs, Kendall C.
Qian, Feng
Zhu, Chuanwu
Arts, Eric J.
Le Grice, Stuart F. J.
Gao, Yong
author_sort Rausch, Jason W.
collection PubMed
description Converting single-stranded viral RNA into double stranded DNA for integration is an essential step in HIV-1 replication. Initial polymerization of minus-strand DNA is primed from a host derived tRNA, whereas subsequent plus-strand synthesis requires viral primers derived from the 3′ and central polypurine tracts (3′ and cPPTs). The 5′ and 3′ termini of these conserved RNA sequence elements are precisely cleaved by RT-associated RNase H to generate specific primers that are used to initiate plus-strand DNA synthesis. In this study, siRNA wad used to produce a replicative HIV-1 variant contained G(-1)A and T(-16)A substitutions within/adjacent to the 3′PPT sequence. Introducing either or both mutations into the 3′PPT region or only the G(-1)A substitution in the cPPT region of NL4-3 produced infectious virus with decreased fitness relative to the wild-type virus. In contrast, introducing the T(-16)A or both mutations into the cPPT rendered the virus(es) incapable of replication, most likely due to the F185L integrase mutation produced by this nucleotide substitution. Finally, the effects of G(-1)A and T(-16)A mutations on cleavage of the 3′PPT were examined using an in vitro RNase H cleavage assay. Substrate containing both mutations was mis-cleaved to a greater extent than either wild-type substrate or substrate containing the T(-16)A mutation alone, which is consistent with the observed effects of the equivalent nucleotide substitutions on the replication fitness of NL4-3 virus. In conclusion, siRNA targeting of the HIV-1 3′PPT region can substantially suppress virus replication, and this selective pressure can be used to generate infectious virus containing mutations within or near the HIV-1 PPT. Moreover, in-depth analysis of the resistance mutations demonstrates that although virus containing a G(-1)A mutation within the 3′PPT is capable of replication, this nucleotide substitution shifts the 3′-terminal cleavage site in the 3′PPT by one nucleotide (nt) and significantly reduces viral fitness.
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spelling pubmed-43931422015-04-21 SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness Rausch, Jason W. Tian, Meijuan Li, Yuejin Angelova, Lora Bagaya, Bernard S. Krebs, Kendall C. Qian, Feng Zhu, Chuanwu Arts, Eric J. Le Grice, Stuart F. J. Gao, Yong PLoS One Research Article Converting single-stranded viral RNA into double stranded DNA for integration is an essential step in HIV-1 replication. Initial polymerization of minus-strand DNA is primed from a host derived tRNA, whereas subsequent plus-strand synthesis requires viral primers derived from the 3′ and central polypurine tracts (3′ and cPPTs). The 5′ and 3′ termini of these conserved RNA sequence elements are precisely cleaved by RT-associated RNase H to generate specific primers that are used to initiate plus-strand DNA synthesis. In this study, siRNA wad used to produce a replicative HIV-1 variant contained G(-1)A and T(-16)A substitutions within/adjacent to the 3′PPT sequence. Introducing either or both mutations into the 3′PPT region or only the G(-1)A substitution in the cPPT region of NL4-3 produced infectious virus with decreased fitness relative to the wild-type virus. In contrast, introducing the T(-16)A or both mutations into the cPPT rendered the virus(es) incapable of replication, most likely due to the F185L integrase mutation produced by this nucleotide substitution. Finally, the effects of G(-1)A and T(-16)A mutations on cleavage of the 3′PPT were examined using an in vitro RNase H cleavage assay. Substrate containing both mutations was mis-cleaved to a greater extent than either wild-type substrate or substrate containing the T(-16)A mutation alone, which is consistent with the observed effects of the equivalent nucleotide substitutions on the replication fitness of NL4-3 virus. In conclusion, siRNA targeting of the HIV-1 3′PPT region can substantially suppress virus replication, and this selective pressure can be used to generate infectious virus containing mutations within or near the HIV-1 PPT. Moreover, in-depth analysis of the resistance mutations demonstrates that although virus containing a G(-1)A mutation within the 3′PPT is capable of replication, this nucleotide substitution shifts the 3′-terminal cleavage site in the 3′PPT by one nucleotide (nt) and significantly reduces viral fitness. Public Library of Science 2015-04-10 /pmc/articles/PMC4393142/ /pubmed/25860884 http://dx.doi.org/10.1371/journal.pone.0122953 Text en https://creativecommons.org/publicdomain/zero/1.0/ This is an open-access article distributed under the terms of the Creative Commons Public Domain declaration, which stipulates that, once placed in the public domain, this work may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose.
spellingShingle Research Article
Rausch, Jason W.
Tian, Meijuan
Li, Yuejin
Angelova, Lora
Bagaya, Bernard S.
Krebs, Kendall C.
Qian, Feng
Zhu, Chuanwu
Arts, Eric J.
Le Grice, Stuart F. J.
Gao, Yong
SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title_full SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title_fullStr SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title_full_unstemmed SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title_short SiRNA-Induced Mutation in HIV-1 Polypurine Tract Region and Its Influence on Viral Fitness
title_sort sirna-induced mutation in hiv-1 polypurine tract region and its influence on viral fitness
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4393142/
https://www.ncbi.nlm.nih.gov/pubmed/25860884
http://dx.doi.org/10.1371/journal.pone.0122953
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