# Circular RNAs and their interactions with RNA-binding proteins to modulate AD-related neuropathology

> **NIH NIH U01** · BOSTON UNIVERSITY MEDICAL CAMPUS · 2024 · $408,750

## Abstract

SUMMARY
New variants, especially in non-coding regions, are expected to be discovered through the ongoing AD
Sequencing Project (ADSP). This proposal will investigate circular RNAs (circRNAs) and RNA binding
proteins (RBPs) that regulate or are regulated by these circRNAs. Recent genomic studies have
discovered thousands of circRNAs produced from both protein-coding genes and non-coding regions of
the genome via a process known as back-splicing. CircRNAs are more enriched in neuronal tissues and
are often derived from genes specific for neuronal and synaptic function. The discovery of these
circRNAs demands a coordinated investigation of RBPs that interact with the circRNAs. Mutations in and
dysfunction of RBPs are known to be major mechanisms contributing to the pathophysiology in
frontotemporal dementia, ALS and AD. However, the contributions of the circRNA:RBP network to these
disease mechanisms are largely unknown. The novel biology of circRNAs opens an entirely new window
into mechanisms of neurodegeneration in ADRD. CircRNAs could contribute to neurodegeneration by
acting as sponges that sequester miRNA/RBPs away from normal mRNA targets, altering splicing or
expression. RBPs also regulate circRNA production by binding to the flanking intronic sequences of
circRNAs which contain many conserved binding sites of splicing factors/RBPs. Thus, sequestration of
RBPs in protein aggregates could cause dysfunctional regulation of circRNAs. The history of genomics
indicate that discovery of each new nucleotide species expands our understanding of disease
mechanisms. The discovery of circRNA presents a major unexplored avenue of RNA metabolism that
demands investigation. We hypothesize that changes in the levels of circRNAs contributes to the
pathophysiology of ADRD, and that discovery of key circRNAs or circRNA-RBP interactions in
aging human brains could uncover novel biomarkers, disease mechanisms or therapeutic
targets. In this proposal, by leveraging large public and our own RNA-seq data (rRNA-depleted), we will
apply several methods to detect and characterize AD-related circRNAs from multiple human brain
regions, and integrate them with ADSP genetic findings (Aim 1). In Aim 2, aside from discovering AD-
related RBPs from human brain RNA-seq, proteomics and ADSP WES/WGS data, we will leverage the
ENCODE CLIP-seq data for RBP binding to identify putative RBP-circRNA interactions with AD, i.e. AD-
related functional RNA elements. Finally, in Aim 3, we will select the top 10% of the circRNAs (~200) and
RBPs (~150) for further high-throughput functional evaluation with a novel, powerful 3D human organoid
model of ADRD, termed AstAD that exhibits the full range of tau pathology and neurodegeneration. We
anticipate that our integrative analyses of ADSP genetics, circRNA, mRNA, RBP and the high-
throughput AstAD functional screen readouts can help generate testable hypothesis for future molecular
mechanisms experimental design.

## Key facts

- **NIH application ID:** 11126150
- **Project number:** 3U01AG072577-04S1
- **Recipient organization:** BOSTON UNIVERSITY MEDICAL CAMPUS
- **Principal Investigator:** Benjamin L Wolozin
- **Activity code:** U01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2024
- **Award amount:** $408,750
- **Award type:** 3
- **Project period:** 2021-07-01 → 2026-06-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/11126150

## Citation

> US National Institutes of Health, RePORTER application 11126150, Circular RNAs and their interactions with RNA-binding proteins to modulate AD-related neuropathology (3U01AG072577-04S1). Retrieved via AI Analytics 2026-06-02 from https://api.ai-analytics.org/grant/nih/11126150. Licensed CC0.

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