# Atoh7 cis regulation and gene regulatory network analysis during retinal ganglion cell development

> **NIH NIH R00** · MEDICAL COLLEGE OF WISCONSIN · 2022 · $248,999

## Abstract

Project Summary/Abstract
Retinal ganglion cells (RGCs) connect the eyes to the brain. They are essential for vertebrate vision and pathogenic targets
in glaucoma. One therapeutic goal of vision scientists is to fully understand the factors required for RGC development, so
these cells can be generated in vitro. The proneural basic helix-loop-helix (bHLH) protein ATOH7 is expressed transiently
in a subpopulation of early retinal progenitor cells, which give rise to the 7 major cell types of the retina but is only
essential as a competence factor for RGC genesis. Loss of ATOH7 causes optic nerve aplasia and severe secondary
retinovascular malformations. Cre-lox lineage data show only 55% of RGCs descend from Atoh7+ progenitors. What
factors control genesis of the other 45% of RGCs? Why do only some Atoh7+ cells become RGCs? In humans with
nonsyndromic congenital retinal nonattachment (NCRNA), a remote 5’ conserved enhancer for ATOH7 is deleted,
preventing development of RGCs and leading to total blindness. This DNA segment is obviously vital, but its exact role is
unknown. In transgene reporter mice, this ‘shadow’ enhancer (SE) appears to be wholly redundant with the ‘primary’
(promoter-adjacent) enhancer (PE), despite is requirement in human NCRNA. In preliminary studies, we observed that
Atoh7 SE deletion mice retain optic nerves. How do these dual enhancer elements coordinately regulate the rapid onset
and offset of Atoh7 expression? Here, we propose to investigate functional differences between the human NCRNA and
mouse SE deletion, to determine how specific DNA sequences control the level, timing and pattern of ATOH7 expression,
to analyze ATOH7 transcriptional repression, and to identify cofactors influencing ATOH7+ cell fate decisions during
RGC genesis. First, we will apply a multi-species approach to test the necessity and sufficiency of each ATOH7
regulatory element and determine precisely how each component contributes to the dynamic tissue and cellular expression
pattern. Second, we will investigate mechanisms of ATOH7 transcriptional repression via Notch effector RPBJ and
Kdm1a, using a high-throughput zebrafish screen, transgenic reporters and RNAseq. Third, we will use single-cell and
pooled ATACseq and RNAseq methods to profile retinal progenitors in detail as they progress through stages of Atoh7
expression. These data will illuminate mechanisms controlling ATOH7 transcription, the onset of retinal neurogenesis and
RGC fate specification; the action of binary enhancers generally; and the potential generation of RGCs in vitro for cell
transplantation. My work toward these goals will be aided by the strong research and career development community at
the University of California, Davis and my established team of mentors. Together, the proposed research and environment
will provide a solid platform for my continued career development as a vision scientist – learning new techniques and
model systems, and interacting with a wide variety ...

## Key facts

- **NIH application ID:** 10480882
- **Project number:** 5R00EY030944-04
- **Recipient organization:** MEDICAL COLLEGE OF WISCONSIN
- **Principal Investigator:** Joel B Miesfeld
- **Activity code:** R00 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2022
- **Award amount:** $248,999
- **Award type:** 5
- **Project period:** 2020-03-01 → 2024-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10480882

## Citation

> US National Institutes of Health, RePORTER application 10480882, Atoh7 cis regulation and gene regulatory network analysis during retinal ganglion cell development (5R00EY030944-04). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10480882. Licensed CC0.

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