HIV latency is reversed by ACSS2-driven histone crotonylation
Guochun Jiang, … , Joseph K. Wong, Satya Dandekar
Guochun Jiang, … , Joseph K. Wong, Satya Dandekar
Published February 19, 2018
Citation Information: J Clin Invest. 2018;128(3):1190-1198. https://doi.org/10.1172/JCI98071.
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Research Article AIDS/HIV Infectious disease

HIV latency is reversed by ACSS2-driven histone crotonylation

Abstract

Eradication of HIV-1 (HIV) is hindered by stable viral reservoirs. Viral latency is epigenetically regulated. While the effects of histone acetylation and methylation at the HIV long-terminal repeat (LTR) have been described, our knowledge of the proviral epigenetic landscape is incomplete. We report that a previously unrecognized epigenetic modification of the HIV LTR, histone crotonylation, is a regulator of HIV latency. Reactivation of latent HIV was achieved following the induction of histone crotonylation through increased expression of the crotonyl-CoA–producing enzyme acyl-CoA synthetase short-chain family member 2 (ACSS2). This reprogrammed the local chromatin at the HIV LTR through increased histone acetylation and reduced histone methylation. Pharmacologic inhibition or siRNA knockdown of ACSS2 diminished histone crotonylation–induced HIV replication and reactivation. ACSS2 induction was highly synergistic in combination with either a protein kinase C agonist (PEP005) or a histone deacetylase inhibitor (vorinostat) in reactivating latent HIV. In the SIV-infected nonhuman primate model of AIDS, the expression of ACSS2 was significantly induced in intestinal mucosa in vivo, which correlated with altered fatty acid metabolism. Our study links the HIV/SIV infection–induced fatty acid enzyme ACSS2 to HIV latency and identifies histone lysine crotonylation as a novel epigenetic regulator for HIV transcription that can be targeted for HIV eradication.

Authors

Guochun Jiang, Don Nguyen, Nancie M. Archin, Steven A. Yukl, Gema Méndez-Lagares, Yuyang Tang, Maher M. Elsheikh, George R. Thompson III, Dennis J. Hartigan-O’Connor, David M. Margolis, Joseph K. Wong, Satya Dandekar

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Figure 5

Early SIV infection induces expression of the fatty acid metabolic gene ACSS2.

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Early SIV infection induces expression of the fatty acid metabolic gene ...
(A) Expression of ACSS2 was induced in the intestinal tissues during early SIV infection. RNA from control (n = 4), acutely SIV-infected (1–2 weeks, n = 4), and chronically SIV-infected (26–28 weeks, n = 6) rhesus macaques was extracted, and expression of ACSS2 was determined by RT-qPCR. ***P < 0.001 versus negative infection; ###P < 0.001 versus acute viral infection. The data were collected from 14 tissue samples and analyzed with 1-way ANOVA. (B and C) Profiles of lipid or fatty acid metabolism products during SIV infection. Metabolomic analysis was performed on the luminal contents from intestinal loops of 10-week SIV-infected (n = 9 in 3 animals) or SIV-negative (n = 9 in 3 animals) rhesus macaques. (D) Viral infection or addition of crotonyl-CoA induces the expression of the fatty acid metabolic enzyme ACSS2, leading to epigenetic regulation of HIV latency/transcription by histone crotonylation. Suppression of ACSS2 by siRNA or AR12 inhibits HIV replication, which may facilitate the establishment of HIV latency.