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PAPγ 通过与 PAXT 核小体 exosome 相互作用来控制 PROMPT ncRNAs 的丰度。

PAPγ associates with PAXT nuclear exosome to control the abundance of PROMPT ncRNAs.

机构信息

CNRS-UMR 9002, Institute of Human Genetics (IGH)/University of Montpellier, Gene Regulation Lab, 34396, Montpellier, France.

Center of Integrative Biology (CBI-CNRS), Molecular, Cellular and Developmental Biology (MCD Unit), University of Toulouse, 31000, Toulouse, France.

出版信息

Nat Commun. 2023 Oct 24;14(1):6745. doi: 10.1038/s41467-023-42620-9.

Abstract

Pervasive transcription of the human genome generates an abundance of RNAs that must be processed and degraded. The nuclear RNA exosome is the main RNA degradation machinery in the nucleus. However, nuclear exosome must be recruited to its substrates by targeting complexes, such as NEXT or PAXT. By proteomic analysis, we identify additional subunits of PAXT, including many orthologs of MTREC found in S. pombe. In particular, we show that polyA polymerase gamma (PAPγ) associates with PAXT. Genome-wide mapping of the binding sites of ZFC3H1, RBM27 and PAPγ shows that PAXT is recruited to the TSS of hundreds of genes. Loss of ZFC3H1 abolishes recruitment of PAXT subunits including PAPγ to TSSs and concomitantly increases the abundance of PROMPTs at the same sites. Moreover, PAPγ, as well as MTR4 and ZFC3H1, is implicated in the polyadenylation of PROMPTs. Our results thus provide key insights into the direct targeting of PROMPT ncRNAs by PAXT at their genomic sites.

摘要

人类基因组的普遍转录产生了大量的 RNA,这些 RNA 必须经过加工和降解。核 RNA 外切酶是细胞核中主要的 RNA 降解机制。然而,核外切酶必须通过靶向复合物(如 NEXT 或 PAXT)被招募到其底物上。通过蛋白质组学分析,我们鉴定了 PAXT 的其他亚基,包括在 S. pombe 中发现的许多 MTREC 的同源物。特别是,我们表明多聚 A 聚合酶 γ(PAPγ)与 PAXT 相关。ZFC3H1、RBM27 和 PAPγ 的结合位点的全基因组图谱显示,PAXT 被招募到数百个基因的 TSS 上。ZFC3H1 的缺失会消除 PAXT 亚基(包括 PAPγ)向 TSS 的募集,同时增加相同位置上 PROMPTs 的丰度。此外,PAPγ 以及 MTR4 和 ZFC3H1 与 PROMPTs 的多聚腺苷酸化有关。因此,我们的研究结果为 PAXT 在其基因组位点上直接靶向 PROMPT ncRNA 提供了关键的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e261/10598014/4f6e62174788/41467_2023_42620_Fig1_HTML.jpg

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