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作为 RNA 靶向 MTREC/PAXT 复合物保守支架的 Red1 的结构分析。

Structural analysis of Red1 as a conserved scaffold of the RNA-targeting MTREC/PAXT complex.

机构信息

Univ. Grenoble Alpes, CNRS, CEA, IBS, F-38000, Grenoble, France.

Institut for Advanced Biosciences, UMR Inserm U1209/CNRS 5309/University Grenoble Alpes, La Tronche, France.

出版信息

Nat Commun. 2022 Aug 24;13(1):4969. doi: 10.1038/s41467-022-32542-3.

Abstract

To eliminate specific or aberrant transcripts, eukaryotes use nuclear RNA-targeting complexes that deliver them to the exosome for degradation. S. pombe MTREC, and its human counterpart PAXT, are key players in this mechanism but inner workings of these complexes are not understood in sufficient detail. Here, we present an NMR structure of an MTREC scaffold protein Red1 helix-turn-helix domain bound to the Iss10 N-terminus and show this interaction is required for proper cellular growth and meiotic mRNA degradation. We also report a crystal structure of a Red1-Ars2 complex explaining mutually exclusive interactions of hARS2 with various ED/EGEI/L motif-possessing RNA regulators, including hZFC3H1 of PAXT, hFLASH or hNCBP3. Finally, we show that both Red1 and hZFC3H1 homo-dimerize via their coiled-coil regions indicating that MTREC and PAXT likely function as dimers. Our results, combining structures of three Red1 interfaces with in vivo studies, provide mechanistic insights into conserved features of MTREC/PAXT architecture.

摘要

为了消除特定或异常的转录本,真核生物利用核 RNA 靶向复合物将其递送至核酶体进行降解。裂殖酵母 MTREC 及其人类对应物 PAXT 是该机制的关键参与者,但这些复合物的内部工作机制尚未得到充分理解。在这里,我们展示了与 Iss10 N 端结合的 MTREC 支架蛋白 Red1 螺旋-转角-螺旋结构域的 NMR 结构,并表明这种相互作用对于正常的细胞生长和减数分裂 mRNA 降解是必需的。我们还报告了 Red1-Ars2 复合物的晶体结构,解释了 hARS2 与各种具有 ED/EGEI/L 基序的 RNA 调节剂(包括 PAXT 的 hZFC3H1、hFLASH 或 hNCBP3)的互斥相互作用。最后,我们表明 Red1 和 hZFC3H1 均可通过其卷曲螺旋区域同源二聚化,这表明 MTREC 和 PAXT 可能作为二聚体发挥作用。我们的结果结合了三个 Red1 界面的结构与体内研究,为 MTREC/PAXT 结构的保守特征提供了机制见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9017/9402713/d088f09494b1/41467_2022_32542_Fig1_HTML.jpg

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