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A-MYB 和 BRDT 依赖性 RNA 聚合酶 II 暂停释放协调哺乳动物减数分裂中的转录调控。

A-MYB and BRDT-dependent RNA Polymerase II pause release orchestrates transcriptional regulation in mammalian meiosis.

机构信息

Baker Institute for Animal Health, College of Veterinary Medicine, Cornell University, Ithaca, NY, 14853, USA.

Department of Biomedical Sciences, College of Veterinary Medicine, Cornell University, Ithaca, NY, 14853, USA.

出版信息

Nat Commun. 2023 Mar 29;14(1):1753. doi: 10.1038/s41467-023-37408-w.

Abstract

During meiotic prophase I, spermatocytes must balance transcriptional activation with homologous recombination and chromosome synapsis, biological processes requiring extensive changes to chromatin state. We explored the interplay between chromatin accessibility and transcription through prophase I of mammalian meiosis by measuring genome-wide patterns of chromatin accessibility, nascent transcription, and processed mRNA. We find that Pol II is loaded on chromatin and maintained in a paused state early during prophase I. In later stages, paused Pol II is released in a coordinated transcriptional burst mediated by the transcription factors A-MYB and BRDT, resulting in ~3-fold increase in transcription. Transcriptional activity is temporally and spatially segregated from key steps of meiotic recombination: double strand breaks show evidence of chromatin accessibility earlier during prophase I and at distinct loci from those undergoing transcriptional activation, despite shared chromatin marks. Our findings reveal mechanisms underlying chromatin specialization in either transcription or recombination in meiotic cells.

摘要

在减数分裂前期 I 中,精母细胞必须平衡转录激活与同源重组和染色体联会,这些生物学过程需要对染色质状态进行广泛的改变。我们通过测量染色质可及性、新生转录和加工 mRNA 的全基因组模式,探索了染色质可及性与转录之间在哺乳动物减数分裂前期 I 中的相互作用。我们发现,Pol II 在前期 I 的早期就被加载到染色质上,并保持暂停状态。在后期,转录因子 A-MYB 和 BRDT 介导的协调转录爆发将暂停的 Pol II 释放出来,导致转录增加约 3 倍。转录活性在时间和空间上与减数分裂重组的关键步骤分离:双链断裂在前期 I 早期显示出染色质可及性的证据,并且与那些发生转录激活的位点不同,尽管它们具有共同的染色质标记。我们的发现揭示了在减数分裂细胞中染色质在转录或重组方面专门化的机制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da3c/10060231/50c157860a68/41467_2023_37408_Fig1_HTML.jpg

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