Stretching muscle cells induces transcriptional and splicing transitions and changes in SR proteins
Alternative splicing is an RNA processing mechanism involved in skeletal muscle development and pathology. Muscular diseases exhibit splicing alterations and changes in mechanobiology leading us to investigate the interconnection between mechanical forces and RNA processing. We performed deep RNA-se...
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Veröffentlicht in: | Communications biology 2022-09, Vol.5 (1), p.987-987, Article 987 |
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Sprache: | eng |
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Zusammenfassung: | Alternative splicing is an RNA processing mechanism involved in skeletal muscle development and pathology. Muscular diseases exhibit splicing alterations and changes in mechanobiology leading us to investigate the interconnection between mechanical forces and RNA processing. We performed deep RNA-sequencing after stretching muscle cells. First, we uncovered transcriptional changes in genes encoding proteins involved in muscle function and transcription. Second, we observed that numerous mechanosensitive genes were part of the MAPK pathway which was activated in response to stretching. Third, we revealed that stretching skeletal muscle cells increased the proportion of alternatively spliced cassette exons and their inclusion. Fourth, we demonstrated that the serine and arginine-rich proteins exhibited stronger transcriptional changes than other RNA-binding proteins and that SRSF4 phosphorylation is mechanosensitive. Identifying SRSF4 as a mechanosensitive RNA-binding protein that might contribute to crosstalk between mechanotransduction, transcription, and splicing could potentially reveal novel insights into muscular diseases, particularly those with unknown etiologies.
Mechanical stretching of skeletal muscle cells induces extensive transcriptional and posttranscriptional changes in genes encoding proteins involved in transcription and muscle cell differentiation. SR proteins also exhibit altered transcription and phosphorylation in response to stretch. |
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ISSN: | 2399-3642 2399-3642 |
DOI: | 10.1038/s42003-022-03915-7 |