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鉴定出一种 E3 连接酶,它在转录应激时靶向 RNA 聚合酶 I 的催化亚基。

Identification of an E3 ligase that targets the catalytic subunit of RNA Polymerase I upon transcription stress.

机构信息

Department of Radiation Oncology and Molecular Radiation Sciences, Johns Hopkins University School of Medicine, Baltimore, Maryland, USA.

Centre for Gene Regulation and Expression, University of Dundee, Dundee, Scotland, United Kingdom.

出版信息

J Biol Chem. 2022 Dec;298(12):102690. doi: 10.1016/j.jbc.2022.102690. Epub 2022 Nov 11.

Abstract

RNA Polymerase I (Pol I) synthesizes rRNA, which is the first and rate-limiting step in ribosome biogenesis. Factors governing the stability of the polymerase complex are not known. Previous studies characterizing Pol I inhibitor BMH-21 revealed a transcriptional stress-dependent pathway for degradation of the largest subunit of Pol I, RPA194. To identify the E3 ligase(s) involved, we conducted a cell-based RNAi screen for ubiquitin pathway genes. We establish Skp-Cullin-F-box protein complex F-box protein FBXL14 as an E3 ligase for RPA194. We show that FBXL14 binds to RPA194 and mediates RPA194 ubiquitination and degradation in cancer cells treated with BMH-21. Mutation analysis in yeast identified lysines 1150, 1153, and 1156 on Rpa190 relevant for the protein degradation. These results reveal the regulated turnover of Pol I, showing that the stability of the catalytic subunit is controlled by the F-box protein FBXL14 in response to transcription stress.

摘要

RNA 聚合酶 I(Pol I)合成 rRNA,这是核糖体生物发生的第一步也是限速步骤。目前尚不清楚控制聚合酶复合物稳定性的因素。先前表征 Pol I 抑制剂 BMH-21 的研究揭示了一种依赖于转录应激的途径,用于降解 Pol I 的最大亚基 RPA194。为了鉴定涉及的 E3 连接酶,我们进行了基于细胞的 RNAi 筛选,以鉴定泛素途径基因。我们确定 Skp-Cullin-F-box 蛋白复合物 F-box 蛋白 FBXL14 是 RPA194 的 E3 连接酶。我们表明,FBXL14 与 RPA194 结合,并在 BMH-21 处理的癌细胞中介导 RPA194 的泛素化和降解。酵母中的突变分析确定了 Rpa190 上与蛋白降解相关的赖氨酸 1150、1153 和 1156。这些结果揭示了 Pol I 的调控性周转,表明在转录应激下,催化亚基的稳定性受 F-box 蛋白 FBXL14 控制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e150/9727647/0bc388ea90de/gr1.jpg

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