# Role of Factor Acetylation in the Regulation of HIV Transcription

> **NIH NIH R37** · J. DAVID GLADSTONE INSTITUTES · 2023 · $621,854

## Abstract

ABSTRACT
Factor acetylation is a recognized epigenetic process governing HIV latency, but the silencing mechanisms
associated with acetylated factors at the latent HIV promoter are not defined. The central hypothesis of this
proposal is that acetyl-lysine reader proteins, such as the bromo- and ET domain-containing BRD4, and the
Regulation of Nuclear Pre-MRNA Domain Containing 1 (RPRD1) proteins are critical regulators of latent HIV
infection. This hypothesis is based on our recent data showing that the short isoform of the BRD4 protein (sBET),
together with the BAF chromatin-remodeling complex, suppresses transcription of HIV and of endogenous
retroviruses, supporting a model in which the sBET-BAF complex senses and silences genome-invading
retroviruses (1). This model is supported by findings implicating another complex of bromodomain and
chromatin-remodeling proteins, the ZYMND8-NuRD complex, in gene silencing during DNA damage (2-4). We
further showed that RPRD1 proteins—without bromodomains—bind acetylated lysines (K7ac) within the RNA
polymerase II, a mark highly enriched at the latent HIV LTR (5, 6). The central hypothesis will be tested in three
specific aims: 1) To define the role of the sBET-BAF complex in genome surveillance. The working hypothesis
is that sBET-BAF, similar to ZMYND8-NURD, senses double-strand DNA breaks caused by integrating
retroviruses and silences gene expression by actively positioning a repressive nucleosome (nuc-1). We will test
the hypothesis by using a dual-fluorescent clone of HIV to analyze sBET-BAF involvement in latency
establishment, by using CRISPR/Cas9 to test dynamics of sBET-BAF recruitment to targeted DNA breaks, and
by using paired-end sequencing to characterize the response of endogenous retroviruses to sBET-BAF
inactivation. 2) To characterize composition and recruitment of sBET-containing complexes. The working
hypothesis is that sBET interacts with multiple chromatin-remodeling complexes to silence incoming retroviruses
and is recruited to the HIV LTR via zinc-finger proteins. Our specific focus is the NuRD nucleosome-remodeling
and deacetylase complex and ZNF592 because of known interactions with sBET and ZMYND8. We will test the
hypothesis in comprehensive mutagenesis, co-immunoprecipitation and chromatin immunoprecipitation
experiments combined with knockdown of select factors. 3) To determine how RPRD1 proteins regulate HIV
transcription. The working hypothesis is that RPRD1 proteins read K7ac marks enriched at the latent HIV
promoter and prevent successful elongation of the paused RNA polymerase II. This hypothesis will be tested in
detailed chromatin immunoprecipitations of CTD modifications at the HIV promoter and with conditional CRISPRi
for RPRD1A/B proteins. As preliminary results implicate RPRD1 proteins in deacetylase recruitment, we will
identify and functionally characterize this deacetylase (6). We expect the proposed work to reveal fundamental
new biology of HIV latency that may ...

## Key facts

- **NIH application ID:** 10655441
- **Project number:** 5R37AI083139-14
- **Recipient organization:** J. DAVID GLADSTONE INSTITUTES
- **Principal Investigator:** Melanie Maria Ott
- **Activity code:** R37 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2023
- **Award amount:** $621,854
- **Award type:** 5
- **Project period:** 2009-07-15 → 2024-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10655441

## Citation

> US National Institutes of Health, RePORTER application 10655441, Role of Factor Acetylation in the Regulation of HIV Transcription (5R37AI083139-14). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10655441. Licensed CC0.

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