# Balancing Erythroid Progenitor Self-Renewal and Differentiation

> **NIH NIH R01** · UNIVERSITY OF WISCONSIN-MADISON · 2020 · $269,676

## Abstract

Project Summary/Abstract
 Genomic technologies have revealed extensive transcription through “non-coding” regions of genomes
to yield regulatory RNAs that control development and physiology. A host of cellular constituents implicated in
regulating RNAs function in broadly expressed multimeric complexes. Many questions remain unanswered
regarding how these complexes control differentiation, proliferation and survival, and how they function in cell
type-specific contexts, e.g. in diverse cells of the hematopoietic system. We discovered that the RNA-
regulatory exosome complex (exosome) opposes primary erythroid cell maturation, and the erythroid
transcription factor GATA-1 represses genes encoding exosome subunits. Downregulating exosome subunits
abrogates intra-complex protein-protein interactions and promotes erythroid maturation. Our progress revealed
the exosome confers expression of the vital receptor tyrosine kinase c-Kit that mediates Stem Cell Factor
(SCF) pro-proliferation signaling in erythroid precursors, while opposing pro-differentiation erythropoietin (Epo)
signals. These results establish a paradigm in which an RNA-regulatory complex orchestrates a
developmental signaling transition to balance proliferation and differentiation. This paradigm has
considerable importance for understanding mechanisms governing erythrocyte genesis in
physiological and pathological states and provides a foundation for devising strategies to control this
process independent of Epo-dependent interventions. In one aim, as specified by SHINE II, we propose
mechanistic/biological analyses to elucidate how the exosome regulates c-Kit expression/function in primary
mouse and human erythroid cells. In Aim 1, we will elucidate how the exosome confers SCF/c-Kit
signaling. Exosome dismantling decreases Kit mRNA and primary transcript levels, the opposite response
predicted from exosome function to degrade RNAs. As the exosome occupies insulators and promoters, is
implicated in superenhancer function and chromatin modification, and suppresses promoter upstream
transcripts that regulate genes, we predict it directly confers Kit transcription (Model 1). Since the exosome
degrades regulatory RNAs, exosome dismantling might elevate regulatory RNA(s) that act in trans to repress
Kit (Model 2). These equally important mechanisms represent a new dimension on how cells mount Stem Cell
Factor (SCF) signaling. In Aim 1a, we will test the hypothesis that direct exosome function at Kit regulates
transcription. In Aim 1b, we will test whether exosome dismantling selectively or broadly expels Pol II and/or its
functionally distinct isoforms. In Aim 1c, we will test whether the mechanism operates in primary human
erythroid cells, which is supported by compelling initial data. These studies will unravel a mechanism governing
acquisition of SCF/c-Kit signaling and how the exosome controls erythroid maturation. Given the crucial c-Kit
functions in normal and malignant hematology, rege...

## Key facts

- **NIH application ID:** 9984388
- **Project number:** 5R01DK113186-03
- **Recipient organization:** UNIVERSITY OF WISCONSIN-MADISON
- **Principal Investigator:** Emery H. Bresnick
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $269,676
- **Award type:** 5
- **Project period:** 2018-08-01 → 2021-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9984388

## Citation

> US National Institutes of Health, RePORTER application 9984388, Balancing Erythroid Progenitor Self-Renewal and Differentiation (5R01DK113186-03). Retrieved via AI Analytics 2026-05-25 from https://api.ai-analytics.org/grant/nih/9984388. Licensed CC0.

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