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在肌生成分化过程中探索高分辨率染色质相互作用变化和肌生成标记基因的功能增强子。

Exploring high-resolution chromatin interaction changes and functional enhancers of myogenic marker genes during myogenic differentiation.

机构信息

Institute of Animal Genetics and Breeding, College of Animal Science and Technology, Sichuan Agricultural University, Chengdu, China.

Jinxin Research Institute for Reproductive Medicine and Genetics, Chengdu Xi'nan Gynecology Hospital Co, Ltd, Chengdu, Sichuan, China.

出版信息

J Biol Chem. 2022 Aug;298(8):102149. doi: 10.1016/j.jbc.2022.102149. Epub 2022 Jul 2.

Abstract

Skeletal muscle differentiation (myogenesis) is a complex and highly coordinated biological process regulated by a series of myogenic marker genes. Chromatin interactions between gene's promoters and their enhancers have an important role in transcriptional control. However, the high-resolution chromatin interactions of myogenic genes and their functional enhancers during myogenesis remain largely unclear. Here, we used circularized chromosome conformation capture coupled with next generation sequencing (4C-seq) to investigate eight myogenic marker genes in C2C12 myoblasts (C2C12-MBs) and C2C12 myotubes (C2C12-MTs). We revealed dynamic chromatin interactions of these marker genes during differentiation and identified 163 and 314 significant interaction sites (SISs) in C2C12-MBs and C2C12-MTs, respectively. The interacting genes of SISs in C2C12-MTs were mainly involved in muscle development, and histone modifications of the SISs changed during differentiation. Through functional genomic screening, we also identified 25 and 41 putative active enhancers in C2C12-MBs and C2C12-MTs, respectively. Using luciferase reporter assays for putative enhancers of Myog and Myh3, we identified eight activating enhancers. Furthermore, dCas9-KRAB epigenome editing and RNA-Seq revealed a role for Myog enhancers in the regulation of Myog expression and myogenic differentiation in the native genomic context. Taken together, this study lays the groundwork for understanding 3D chromatin interaction changes of myogenic genes during myogenesis and provides insights that contribute to our understanding of the role of enhancers in regulating myogenesis.

摘要

骨骼肌分化(成肌分化)是一个复杂而高度协调的生物学过程,受一系列成肌标记基因的调节。基因启动子与其增强子之间的染色质相互作用在转录调控中起着重要作用。然而,成肌基因及其功能增强子在成肌过程中的高分辨率染色质相互作用在很大程度上仍不清楚。在这里,我们使用圆形染色体构象捕获与下一代测序(4C-seq)技术研究了 C2C12 成肌细胞(C2C12-MBs)和成肌管(C2C12-MTs)中的八个成肌标记基因。我们揭示了这些标记基因在分化过程中的动态染色质相互作用,并分别在 C2C12-MBs 和 C2C12-MTs 中鉴定了 163 个和 314 个显著相互作用位点(SISs)。C2C12-MTs 中 SIS 的相互作用基因主要参与肌肉发育,并且 SIS 的组蛋白修饰在分化过程中发生变化。通过功能基因组筛选,我们还分别在 C2C12-MBs 和 C2C12-MTs 中鉴定了 25 个和 41 个可能的活性增强子。使用荧光素酶报告基因检测 Myog 和 Myh3 的潜在增强子,我们鉴定了八个激活增强子。此外,dCas9-KRAB 表观基因组编辑和 RNA-Seq 揭示了 Myog 增强子在调节 Myog 表达和成肌分化中的作用在天然基因组背景下。总之,这项研究为理解成肌过程中成肌基因的 3D 染色质相互作用变化奠定了基础,并为我们理解增强子在调节成肌中的作用提供了新的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cef1/9352921/689046b27ce8/gr1.jpg

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