# Regulation of Dnmt3 Activity at Enhancers of Cell Identity Genes During Differentiation

> **NIH NIH R01** · PURDUE UNIVERSITY · 2021 · $320,435

## Abstract

Project Summary
Maintenance of proper patterns of DNA methylation is essential for the integrity of cell identity, failure of which
results in aberrant activation of genes, which in turn modulates signaling pathways leading to cancer and de-
velopmental disorders. Despite a large body of evidence supporting the role of aberrant DNA methylation in
etiology of several human diseases, the fundamental mechanisms that regulate the target site specificity of the
de novo DNA MTases, Dnmt3a and 3b, are largely unknown. Gene repression is an orchestrated event that
involves loss of coactivator complexes from the regulatory elements and changes in chromatin state including
gain of DNA methylation, resulting in stable gene repression. Recent studies have enumerated the role of en-
hancer-mediated regulation of oncogenes in various cancers. Others have shown aberrant expression of plu-
ripotency genes mediates dedifferentiation in several cancers. Changes in the chromatin state of the enhanc-
ers of pluripotency genes have been shown to be critical for the repression of pluripotency genes during mu-
rine embryonic stem cell (ESC) differentiation. The role of DNA methylation in this process and the mechanism
that targets DNA methylation to the enhancers during differentiation have not been addressed. Understanding
the fundamental epigenetic mechanisms involved in the establishment of enhancer-mediated pluripotency (Pp)
gene repression during normal cell differentiation will, in the long-term, lead to development of therapeutic
strategies to restore Pp gene repression in cancer cells. Our objective in this application is to elucidate molecu-
lar mechanism(s) that regulate the activity of Dnmt3a and 3b at enhancers of Pp genes genome-wide using
ESC differentiation as a model system. Supported by our strong preliminary data and recently published stud-
ies on the dynamics of the chromatin state of Pp gene enhancers, we will test our hypothesis that Lsd1-
Mi2/NURD activity acts as an epigenetic switch at Pp gene enhancers to activate Dnmt3 enzymes, causing
site-specific DNA methylation and stable Pp gene repression. We will further elucidate the role of chromatin
conformation in facilitating enhancer-targeted activity of Dnmt3a and/or 3b to specific promoters during the ear-
ly phase of ESC differentiation. To test if both Dnmt3a and 3b are regulated by these mechanisms, we will map
their genome-wide activity during ESC differentiation. Our rationale for these studies is that their successful
completion is expected to fill the gap in our understanding of how the epigenetic “cross talk” mechanisms, dur-
ing cell differentiation, modulate Dnmt3a/3b activity to terminate the pluripotency program, disruption of which
could lead to developmental disorders and cancer. Additionally, the outcomes from these studies are expected
to provide new insights into how the interplay between various epigenetic factors affects gene expression, con-
tributing to phenotypic variation...

## Key facts

- **NIH application ID:** 10202637
- **Project number:** 5R01GM118654-05
- **Recipient organization:** PURDUE UNIVERSITY
- **Principal Investigator:** Humaira Gowher
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2021
- **Award amount:** $320,435
- **Award type:** 5
- **Project period:** 2017-07-01 → 2024-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10202637

## Citation

> US National Institutes of Health, RePORTER application 10202637, Regulation of Dnmt3 Activity at Enhancers of Cell Identity Genes During Differentiation (5R01GM118654-05). Retrieved via AI Analytics 2026-05-27 from https://api.ai-analytics.org/grant/nih/10202637. Licensed CC0.

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