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U6 snRNA 特异性末端尿苷酰转移酶的晶体结构。

Crystal structures of U6 snRNA-specific terminal uridylyltransferase.

机构信息

Department of Computational Biology and Medical Sciences, Graduate School of Frontier Sciences, the University of Tokyo, Kashiwa, Chiba 277-8562, Japan.

National Institute of Advanced Industrial Science and Technology, Biomedical Research Institute, 1-1-1 Higashi, Tsukuba, Ibaraki 305-8566, Japan.

出版信息

Nat Commun. 2017 Jun 7;8:15788. doi: 10.1038/ncomms15788.

Abstract

The terminal uridylyltransferase, TUT1, builds or repairs the 3'-oligo-uridylylated tail of U6 snRNA. The 3'-oligo-uridylylated tail is the Lsm-binding site for U4/U6 di-snRNP formation and U6 snRNA recycling for pre-mRNA splicing. Here, we report crystallographic and biochemical analyses of human TUT1, which revealed the mechanisms for the specific uridylylation of the 3'-end of U6 snRNA by TUT1. The O and O atoms of the UTP base form hydrogen bonds with the conserved His and Asn in the catalytic pocket, respectively, and TUT1 preferentially incorporates UMP onto the 3'-end of RNAs. TUT1 recognizes the entire U6 snRNA molecule by its catalytic domains, N-terminal RNA-recognition motifs and a previously unidentified C-terminal RNA-binding domain. Each domain recognizes specific regions within U6 snRNA, and the recognition is coupled with the domain movements and U6 snRNA structural changes. Hence, TUT1 functions as the U6 snRNA-specific terminal uridylyltransferase required for pre-mRNA splicing.

摘要

末端尿嘧啶转移酶 TUT1 构建或修复 U6 snRNA 的 3'-寡尿嘧啶化尾巴。3'-寡尿嘧啶化尾巴是 Lsm 结合位点,用于 U4/U6 二-snRNP 的形成和 U6 snRNA 的循环利用,以进行 pre-mRNA 剪接。在这里,我们报告了人源 TUT1 的晶体结构和生化分析,揭示了 TUT1 特异性尿嘧啶核苷酰化 U6 snRNA 3'末端的机制。UTP 碱基的 O 和 O 原子分别与催化口袋中的保守 His 和 Asn 形成氢键,并且 TUT1 优先将 UMP 掺入到 RNA 的 3'末端。TUT1 通过其催化结构域、N 端 RNA 识别基序和先前未识别的 C 端 RNA 结合结构域识别整个 U6 snRNA 分子。每个结构域识别 U6 snRNA 中的特定区域,并且识别与结构域运动和 U6 snRNA 结构变化相关联。因此,TUT1 作为 pre-mRNA 剪接所需的 U6 snRNA 特异性末端尿嘧啶转移酶发挥作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6b74/5467268/921cf28b750e/ncomms15788-f1.jpg

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