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In heart failure reactivation of RNA-binding proteins is associated with the expression of 1,523 fetal-specific isoforms

基因亚型 生物 选择性拼接 心力衰竭 转录组 胎儿 心脏发育 RNA剪接 基因表达 细胞生物学
作者
Matteo D’Antonio,Jennifer Nguyen,Timothy D. Arthur,Hiroko Matsui,Margaret K.R. Donovan,Agnieszka D'Antonio-Chronowska,Kelly A. Frazer
出处
期刊:PLOS Computational Biology [Public Library of Science]
卷期号:18 (2): e1009918-e1009918
标识
DOI:10.1371/journal.pcbi.1009918
摘要

Reactivation of fetal-specific genes and isoforms occurs during heart failure. However, the underlying molecular mechanisms and the extent to which the fetal program switch occurs remains unclear. Limitations hindering transcriptome-wide analyses of alternative splicing differences (i.e. isoform switching) in cardiovascular system (CVS) tissues between fetal, healthy adult and heart failure have included both cellular heterogeneity across bulk RNA-seq samples and limited availability of fetal tissue for research. To overcome these limitations, we have deconvoluted the cellular compositions of 996 RNA-seq samples representing heart failure, healthy adult (heart and arteria), and fetal-like (iPSC-derived cardiovascular progenitor cells) CVS tissues. Comparison of the expression profiles revealed that reactivation of fetal-specific RBPs, and the accompanied re-expression of 1,523 fetal-specific isoforms, contribute to the transcriptome differences between heart failure and healthy adult heart. Of note, isoforms for 20 different RBPs were among those that reverted in heart failure to the fetal-like expression pattern. We determined that, compared with adult-specific isoforms, fetal-specific isoforms encode proteins that tend to have more functions, are more likely to harbor RBP binding sites, have canonical sequences at their splice sites, and contain typical upstream polypyrimidine tracts. Our study suggests that compared with healthy adult, fetal cardiac tissue requires stricter transcriptional regulation, and that during heart failure reversion to this stricter transcriptional regulation occurs. Furthermore, we provide a resource of cardiac developmental stage-specific and heart failure-associated genes and isoforms, which are largely unexplored and can be exploited to investigate novel therapeutics for heart failure.
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