# Mechanisms of Homeodomain Transcriptional Specificity

> **NIH NIH R01** · CINCINNATI CHILDRENS HOSP MED CTR · 2022 · $59,635

## Abstract

PROJECT ABSTRACT
Homeodomain (HD) proteins comprise a large family of transcription factors (TFs) that regulate numerous
aspects of animal development. For example, members of the Hox-like (HoxL) and Nkx-like (NKL) HD proteins
regulate processes ranging from patterning of the anterior-posterior axis (A-P) of the embryo to specifying
individual cell fates within different organ systems. Intriguingly, the HoxL and NKL proteins have highly similar
HDs that bind largely overlapping AT-rich DNA sequences in vitro. These findings provide a classic TF specificity
paradox: How do TFs with highly similar in vitro DNA binding activities achieve sufficient in vivo specificity to
ensure the accurate regulation of genetic programs in different cell types? To address this paradox, my lab is
focused on defining how HD TFs achieve in vivo specificity by forming cooperative TF complexes on cis-
regulatory modules. Our preliminary and published data reveal that members of the HoxL and NKL TFs differ in
their ability to form homo- and heterodimer TF complexes on DNA. For instance, we unexpectedly found that the
Gsx/Ind TFs, which specify neuronal cell fates in animals from flies to mammals, differentially regulate gene
expression when bound to DNA as monomers versus homodimers. In contrast, the Abdominal-A (Abd-A) Hox
TF, which specifies distinct cell fates in the Drosophila abdomen, does not bind DNA as a homodimer, but instead
cooperatively binds DNA with three other HD proteins: Extradenticle (Exd), Homothorax (Hth), and Engrailed
(En). These data support the hypothesis that HD TFs achieve target and regulatory specificity by binding distinct
combinations of AT-rich DNA sites as monomers, cooperative homodimers, or cooperative heterodimers. To test
this hypothesis, we propose two aims: In Aim1, we propose to determine how HD monomer versus homodimer
binding impacts target gene binding and regulation. To achieve this goal, we will (1) systematically define which
HoxL and NKL HDs cooperatively bind DNA as homodimers; (2) assess the regulatory potential of each HD on
monomer vs dimer sites in cell culture assays; and (3) define the mechanism and function of Ind homodimer
formation on Drosophila neuroblast gene expression using structural biology and transgenic reporter,
CUT&RUN, and RNA-seq assays. In Aim2, we propose to define how the choice of Hox heterodimer partner
impacts the DNA binding and regulatory specificity of the Abd-A Hox TF. To achieve this goal, we will (1) define
the DNA motifs and molecular domains required for cooperative Abd-A/Hth and Abd-A/En complexes; (2) test
the role of Abd-A heterodimerization domains in gene activation and repression assays in the Drosophila embryo;
(3) define the in vivo binding motifs and target genes regulated by Abd-A with a focus on identifying heterodimer
binding events using CUT&RUN and RNA-seq assays. Since the TFs and biological processes studied are highly
conserved between flies and mammals, we are optimistic o...

## Key facts

- **NIH application ID:** 10673333
- **Project number:** 3R01GM079428-12S1
- **Recipient organization:** CINCINNATI CHILDRENS HOSP MED CTR
- **Principal Investigator:** BRIAN GEBELEIN
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2022
- **Award amount:** $59,635
- **Award type:** 3
- **Project period:** 2008-04-01 → 2024-07-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10673333

## Citation

> US National Institutes of Health, RePORTER application 10673333, Mechanisms of Homeodomain Transcriptional Specificity (3R01GM079428-12S1). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10673333. Licensed CC0.

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