# Project 3: Use of an IRES-driven N-truncated dystrophin isoform as a clinical therapy for 5 mutations in the dystrophinopathies

> **NIH NIH P50** · RESEARCH INST NATIONWIDE CHILDREN'S HOSP · 2020 · $299,585

## Abstract

Project 3 (Flanigan) 
Abstract 
Duchenne muscular dystrophy (DMD) typically results from mutations in the DMD gene that 
disrupt the open reading frame, resulting in no dystrophin protein, whereas the milder Becker 
muscular dystrophy (BMD) typically results from mutations that allow expression of a partially 
functional dystrophin protein. Among the exceptions to this rule are people with mutations in the 
first few exons of the gene would be predicted to result in DMD but instead are very mild BMD 
or are even asymptomatic. We have recently shown that this is due to translation of an N- 
truncated dystrophin which we call ΔCH1, and which results from a cap-independent 
translational process mediated by a newly described internal ribosome entry site (IRES) within 
exon 5. We have recently shown that we can activate the IRES by skipping exon 2 using an 
adeno-associate virus (AAV)-U7snRNA approach, or by antisense oligomer-mediated exon 
skipping. Our long-term goal is to develop exon 2 skipping as a therapy for patients who carry a 
duplication of exon 2, which is the most common single exon duplication in DMD patients, as 
well as for other mutations within the first few exons of the gene. To study this, we have 
developed a new mouse model of DMD that contains an exon 2 duplication (the Dup2 mouse) 
and have used it to generate extensive preclinical data showing that AAV-mediated delivery of a 
modified U7snRNA targeting exon 2 works very well. Our objective in this project is to broaden 
the applicability of this approach, and to test other ways to stimulated the IRES, as inducing 
expression would be a meaningful therapeutic approach for up to 5% of dystrophinopathy 
patients. Under Aim 1, we will assess exon 2 skipping and IRES activation using 
phosphorodiamidate morpholino oligomers (PMOs) provided by Sarepta Therapeutics. Under 
Aim 2, we will seek to validate small molecule activators of the dystrophin IRES identified in a 
high-throughput screen at PTC Therapeutics. Under Aim 3, we will develop a develop a 
muscle-specific AAV-mediated CRISPR/Cas9 approach to induce somatic IRES activation. As 
we have already demonstrated the proof-of-concept of IRES activation using an 
AAV9.U7snRNA approach to exon 2 skipping, the expected outcome will be to demonstrate the 
broader applicability of our approach to 5' mutations using complementary methods directed at 
both splicing and translational modification strategies. The immediate impact of our work will be 
to provide preclinical data that supports rapid clinical development of therapies to provide a 
clinically meaningful benefit to boys with DMD and BMD, which will be facilitated by our 
established collaborations with biopharmaceutical companies and by our own extensive 
experience in investigator-initiated pre-IND interactions

## Key facts

- **NIH application ID:** 10017028
- **Project number:** 5P50AR070604-05
- **Recipient organization:** RESEARCH INST NATIONWIDE CHILDREN'S HOSP
- **Principal Investigator:** KEVIN M FLANIGAN
- **Activity code:** P50 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $299,585
- **Award type:** 5
- **Project period:** 2016-09-14 → 2022-08-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10017028

## Citation

> US National Institutes of Health, RePORTER application 10017028, Project 3: Use of an IRES-driven N-truncated dystrophin isoform as a clinical therapy for 5 mutations in the dystrophinopathies (5P50AR070604-05). Retrieved via AI Analytics 2026-05-22 from https://api.ai-analytics.org/grant/nih/10017028. Licensed CC0.

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