Literature DB >> 35990589

ATAC-Seq of a Single Myofiber from Mus musculus.

Korin Sahinyan1,2, Darren M Blackburn1,2, Vahab D Soleimani1,2.   

Abstract

Chromatin accessibility is a key determinant of gene expression that can be altered under different physiological and disease conditions. Skeletal muscle is made up of myofibers that are highly plastic and adaptive. Therefore, assessing the genome-wide chromatin state of myofibers under various conditions is very important to gain insight into the epigenetic state of myonuclei. The rigid nature of myofibers, as well as the low number of myonuclei that they contain, have rendered genome-wide studies with myofibers challenging. In recent years, ATAC-Seq from whole muscle and single nucleus ATAC-Seq have been performed. However, these techniques cannot distinguish between different fiber and cell types present in the muscle. In addition, due to the limited depth capacity obtained from single nucleus ATAC-Seq, an extensive comparative analysis cannot be performed. Here, we introduce a protocol where we combine the isolation of a single myofiber with OMNI ATAC-Seq. This protocol allows for genome-wide analysis of accessible chromatin regions of a selected single myofiber at a sufficient depth for comparative analysis under various physiological and disease conditions. This protocol can also allow for a specific myofiber to be selected, such as a regenerating myofiber. In the future, this protocol can help identify global changes in chromatin state under various conditions, as well as between different types of myofibers. Graphical abstract.
Copyright © The Authors; exclusive licensee Bio-protocol LLC.

Entities:  

Keywords:  ATAC-Seq ; Chromatin Accessibility ; Epigenetics ; Single myofiber ; Skeletal Muscle

Year:  2022        PMID: 35990589      PMCID: PMC9362843          DOI: 10.21769/BioProtoc.4452

Source DB:  PubMed          Journal:  Bio Protoc        ISSN: 2331-8325


  15 in total

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6.  Application of ATAC-Seq for genome-wide analysis of the chromatin state at single myofiber resolution.

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9.  Myf6/MRF4 is a myogenic niche regulator required for the maintenance of the muscle stem cell pool.

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