Bulk and single‐cell alternative splicing analyses reveal roles of TRA2B in myogenic differentiation

Author:

Chen Genghua123ORCID,Chen Jiahui123,Qi Lin123,Yin Yunqian123,Lin Zetong123,Wen Huaqiang123,Zhang Shuai123,Xiao Chuanyun4,Bello Semiu Folaniyi123ORCID,Zhang Xiquan123,Nie Qinghua123,Luo Wen123

Affiliation:

1. College of Animal Science South China Agricultural University Guangzhou Guangdong China

2. Guangdong Provincial Key Lab of Agro‐Animal Genomics and Molecular Breeding, Lingnan Guangdong Laboratory of Modern Agriculture & State Key Laboratory for Conservation and Utilization of Subtropical Agro‐Bioresources, Key Laboratory of Chicken Genetics, Breeding and Reproduction, Ministry of Agriculture Guangzhou Guangdong China

3. State Key Laboratory of Livestock and Poultry Breeding, and Lingnan Guangdong Laboratory of Agriculture South China Agricultural University Guangzhou China

4. Human and Animal Physiology Wageningen University Wageningen The Netherlands

Abstract

AbstractAlternative splicing (AS) disruption has been linked to disorders of muscle development, as well as muscular atrophy. However, the precise changes in AS patterns that occur during myogenesis are not well understood. Here, we employed isoform long‐reads RNA‐seq (Iso‐seq) and single‐cell RNA‐seq (scRNA‐seq) to investigate the AS landscape during myogenesis. Our Iso‐seq data identified 61,146 full‐length isoforms representing 11,682 expressed genes, of which over 52% were novel. We identified 38,022 AS events, with most of these events altering coding sequences and exhibiting stage‐specific splicing patterns. We identified AS dynamics in different types of muscle cells through scRNA‐seq analysis, revealing genes essential for the contractile muscle system and cytoskeleton that undergo differential splicing across cell types. Gene‐splicing analysis demonstrated that AS acts as a regulator, independent of changes in overall gene expression. Two isoforms of splicing factor TRA2B play distinct roles in myogenic differentiation by triggering AS of TGFBR2 to regulate canonical TGF‐β signalling cascades differently. Our study provides a valuable transcriptome resource for myogenesis and reveals the complexity of AS and its regulation during myogenesis.

Funder

National Key Research and Development Program of China

Publisher

Wiley

Subject

Cell Biology,General Medicine

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