Rescue of Scn5a mis-splicing does not improve the structural and functional heart defects of a DM1 heart mouse model.

IF 3.1 2区 生物学 Q3 BIOCHEMISTRY & MOLECULAR BIOLOGY Human molecular genetics Pub Date : 2024-10-07 DOI:10.1093/hmg/ddae117
Larissa Nitschke, Rong-Chi Hu, Andrew N Miller, Thomas A Cooper
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Abstract

Myotonic Dystrophy Type 1 (DM1) is an autosomal dominant multisystemic disorder for which cardiac features, including conduction delays and arrhythmias, are the second leading cause of disease mortality. DM1 is caused by expanded CTG repeats in the 3' untranslated region of the DMPK gene. Transcription of the expanded DMPK allele produces mRNAs containing long tracts of CUG repeats, which sequester the Muscleblind-Like family of RNA binding proteins, leading to their loss-of-function and the dysregulation of alternative splicing. A well-characterized mis-regulated splicing event in the DM1 heart is the increased inclusion of SCN5A exon 6A rather than the mutually exclusive exon 6B that normally predominates in adult heart. As previous work showed that forced inclusion of Scn5a exon 6A in mice recapitulates cardiac DM1 phenotypes, we tested whether rescue of Scn5a mis-splicing would improve the cardiac phenotypes in a DM1 heart mouse model. We generated mice lacking Scn5a exon 6A to force the expression of the adult SCN5A isoform including exon 6B and crossed these mice to our previously established CUG960 DM1 heart mouse model. We showed that correction Scn5a mis-splicing does not improve the DM1 heart conduction delays and structural changes induced by CUG repeat RNA expression. Interestingly, we found that in addition to Scn5a mis-splicing, Scn5a expression is reduced in heart tissues of CUG960 mice and DM1-affected individuals. These data indicate that Scn5a mis-splicing is not the sole driver of DM1 heart deficits and suggest a potential role for reduced Scn5a expression in DM1 cardiac disease.

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挽救 Scn5a 的错误剪接并不能改善 DM1 心脏小鼠模型的心脏结构和功能缺陷。
肌营养不良症 1 型(DM1)是一种常染色体显性多系统疾病,其心脏特征(包括传导延迟和心律失常)是导致该病死亡的第二大原因。DM1 由 DMPK 基因 3' 非翻译区中的扩展 CTG 重复序列引起。扩增的 DMPK 等位基因转录产生的 mRNA 含有长长的 CUG 重复序列,这些重复序列将 RNA 结合蛋白 Muscleblind-Like 家族封闭起来,导致其功能丧失和替代剪接失调。在DM1心脏中,一个特征明确的剪接失调事件是SCN5A外显子6A的包含增加,而不是成人心脏中通常占主导地位的互斥外显子6B。之前的研究表明,小鼠Scn5a外显子6A的强迫包含可重现DM1心脏表型,因此我们测试了拯救Scn5a错误剪接是否能改善DM1心脏小鼠模型的心脏表型。我们生成了缺乏 Scn5a 6A 外显子的小鼠,以强制表达包括 6B 外显子在内的成年 SCN5A 异构体,并将这些小鼠与我们之前建立的 CUG960 DM1 心脏小鼠模型杂交。我们发现,纠正 Scn5a 的错误拼接并不能改善 CUG 重复 RNA 表达引起的 DM1 心脏传导延迟和结构变化。有趣的是,我们发现除了 Scn5a 的错误剪接外,Scn5a 在 CUG960 小鼠和 DM1 受影响个体的心脏组织中的表达也降低了。这些数据表明,Scn5a的错误剪接并不是DM1心脏缺陷的唯一驱动因素,并提示了Scn5a表达的减少在DM1心脏疾病中的潜在作用。
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来源期刊
Human molecular genetics
Human molecular genetics 生物-生化与分子生物学
CiteScore
6.90
自引率
2.90%
发文量
294
审稿时长
2-4 weeks
期刊介绍: Human Molecular Genetics concentrates on full-length research papers covering a wide range of topics in all aspects of human molecular genetics. These include: the molecular basis of human genetic disease developmental genetics cancer genetics neurogenetics chromosome and genome structure and function therapy of genetic disease stem cells in human genetic disease and therapy, including the application of iPS cells genome-wide association studies mouse and other models of human diseases functional genomics computational genomics In addition, the journal also publishes research on other model systems for the analysis of genes, especially when there is an obvious relevance to human genetics.
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