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RNA 结合蛋白和热休克蛋白 90 是细胞质加帽酶相互作用组的组成部分。

RNA-binding proteins and heat-shock protein 90 are constituents of the cytoplasmic capping enzyme interactome.

机构信息

From the Center for RNA Biology.

Ohio State Biochemistry Program.

出版信息

J Biol Chem. 2018 Oct 26;293(43):16596-16607. doi: 10.1074/jbc.RA118.004973. Epub 2018 Aug 30.

DOI:10.1074/jbc.RA118.004973
PMID:30166341
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6204893/
Abstract

The -methylguanosine cap is added in the nucleus early in gene transcription and is a defining feature of eukaryotic mRNAs. Mammalian cells also possess cytoplasmic machinery for restoring the cap at uncapped or partially degraded RNA 5' ends. Central to both pathways is capping enzyme (CE) (RNA guanylyltransferase and 5'-phosphatase (RNGTT)), a bifunctional, nuclear and cytoplasmic enzyme. CE is recruited to the cytoplasmic capping complex by binding of a C-terminal proline-rich sequence to the third Src homology 3 (SH3) domain of NCK adapter protein 1 (NCK1). To gain broader insight into the cellular context of cytoplasmic recapping, here we identified the protein interactome of cytoplasmic CE in human U2OS cells through two complementary approaches: chemical cross-linking and recovery with cytoplasmic CE and protein screening with proximity-dependent biotin identification (BioID). This strategy unexpectedly identified 66 proteins, 52 of which are RNA-binding proteins. We found that CE interacts with several of these proteins independently of RNA, mediated by sequences within its N-terminal triphosphatase domain, and we present a model describing how CE-binding proteins may function in defining recapping targets. This analysis also revealed that CE is a client protein of heat shock protein 90 (HSP90). Nuclear and cytoplasmic CEs were exquisitely sensitive to inhibition of HSP90, with both forms declining significantly following treatment with each of several HSP90 inhibitors. Importantly, steady-state levels of capped mRNAs decreased in cells treated with the HSP90 inhibitor geldanamycin, raising the possibility that the cytotoxic effect of these drugs may partially be due to a general reduction in translatable mRNAs.

摘要

-mG 帽在基因转录的早期在核内被添加,是真核 mRNA 的一个特征。哺乳动物细胞也拥有细胞质机制来恢复无帽或部分降解的 RNA 5'端的帽。两条途径的核心都是帽酶(CE)(RNA 鸟苷转移酶和 5'-磷酸酶(RNGTT)),一种具有双功能的核质酶。CE 通过其 C 端富含脯氨酸的序列与 NCK 衔接蛋白 1(NCK1)的第三个Src 同源 3(SH3)结构域结合,被募集到细胞质加帽复合物中。为了更深入地了解细胞质加帽的细胞环境,我们通过两种互补的方法鉴定了人 U2OS 细胞中细胞质 CE 的蛋白质相互作用组:化学交联和细胞质 CE 的回收以及邻近依赖性生物素鉴定(BioID)的蛋白质筛选。这种策略出人意料地鉴定了 66 种蛋白质,其中 52 种是 RNA 结合蛋白。我们发现,CE 与其中几种蛋白质相互作用,与 RNA 无关,由其 N 端三磷酸酶结构域内的序列介导,我们提出了一个模型,描述了 CE 结合蛋白如何在定义加帽靶标中发挥作用。该分析还表明,CE 是热休克蛋白 90(HSP90)的客户蛋白。核质和细胞质 CE 对 HSP90 的抑制极为敏感,在用几种 HSP90 抑制剂中的每一种处理后,两种形式的 CE 都显著下降。重要的是,用 HSP90 抑制剂格尔德霉素处理的细胞中,有帽 mRNA 的稳态水平下降,这增加了这些药物的细胞毒性可能部分是由于可翻译的 mRNA 普遍减少的可能性。

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引用本文的文献

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Inhibition of cytoplasmic cap methylation identifies 5' TOP mRNAs as recapping targets and reveals recapping sites downstream of native 5' ends.抑制细胞质帽甲基化可识别 5' TOP mRNAs 作为再帽化靶标,并揭示天然 5' 末端下游的再帽化位点。
Nucleic Acids Res. 2020 Apr 17;48(7):3806-3815. doi: 10.1093/nar/gkaa046.
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mRNA 5' ends targeted by cytoplasmic recapping cluster at CAGE tags and select transcripts are alternatively spliced.细胞质重帽簇靶向 CAGE 标签的 mRNA 5' 端,并选择性剪接部分转录本。
FEBS Lett. 2019 Apr;593(7):670-679. doi: 10.1002/1873-3468.13349. Epub 2019 Mar 9.

本文引用的文献

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The Human RNA-Binding Proteome and Its Dynamics during Translational Arrest.人类 RNA 结合蛋白组及其在翻译停滞时的动态变化。
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RNA guanine-7 methyltransferase catalyzes the methylation of cytoplasmically recapped RNAs.RNA鸟嘌呤-7甲基转移酶催化细胞质中重新加帽的RNA的甲基化。
Nucleic Acids Res. 2017 Oct 13;45(18):10726-10739. doi: 10.1093/nar/gkx801.
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Capping Enzyme mRNA-cap/RNGTT Regulates Hedgehog Pathway Activity by Antagonizing Protein Kinase A.帽结合酶 mRNA-帽/RNGTT 通过拮抗蛋白激酶 A 调节 Hedgehog 途径活性。
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