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自剪接II组内含子催化效应结构域5的结构:与剪接体U6 RNA的相似性

Structure of a self-splicing group II intron catalytic effector domain 5: parallels with spliceosomal U6 RNA.

作者信息

Seetharaman Mahadevan, Eldho Nadukkudy V, Padgett Richard A, Dayie Kwaku T

机构信息

Department of Molecular Genetics, Lerner Research Institute, Cleveland Clinic Foundation, Cleveland, OH 44195, USA.

出版信息

RNA. 2006 Feb;12(2):235-47. doi: 10.1261/rna.2237806.

Abstract

Domain 5 (D5) is absolutely required for all catalytic functions of group II introns. Here we describe the solution NMR structure, electrostatic calculations, and detailed magnesium ion-binding surface of D5 RNA from the Pylaiella littoralis large ribosomal RNA intron (D5-PL). The overall structure consists of a hairpin capped by a GNRA tetraloop. The stem is divided into lower and upper helices of 8 and 5 bp, respectively, separated by an internal bulge. The D5-PL internal bulge nucleotides stack into the helical junction, resulting in a coupling between the bulge A25 and the closing base pair (G8-C27) of the lower helix. Comparison of the D5-PL structure to previously reported related structures indicates that our structure is most similar, in the helical regions, to the crystal structure of D5 from yeast Ai5gamma (D5-Ai5gamma) and the NMR structure of the U6 snRNA stem-loop region. Our structure differs in many respects from both the NMR and X-ray structures of D5-Ai5gamma in the bulge region. Electrostatic calculations and NMR chemical shift perturbation analyses reveal magnesium ion-binding sites in the tetraloop, internal bulge, and the AGC triad in the lower stem. Our results suggest that the structure, electrostatic environment, and the magnesium ion-binding sites within the tetraloop, bulge, and triad regions are conserved features of the splicing machinery of both the group II introns and the spliceosome that are likely key for catalytic function.

摘要

结构域5(D5)对于II类内含子的所有催化功能来说是绝对必需的。在此,我们描述了来自滨海 pylaiella 大核糖体RNA内含子的D5 RNA(D5-PL)的溶液核磁共振结构、静电计算以及详细的镁离子结合表面。其整体结构由一个由GNRA四环封闭的发夹组成。茎干分为分别含有8个和5个碱基对的下部和上部螺旋,由一个内部凸起隔开。D5-PL内部凸起的核苷酸堆积到螺旋连接处,导致凸起A25与下部螺旋的封闭碱基对(G8-C27)之间产生耦合。将D5-PL结构与先前报道的相关结构进行比较表明,在螺旋区域,我们的结构与来自酵母Ai5γ的D5的晶体结构(D5-Ai5γ)以及U6 snRNA茎环区域的核磁共振结构最为相似。在凸起区域,我们的结构在许多方面与D5-Ai5γ的核磁共振和X射线结构都不同。静电计算和核磁共振化学位移扰动分析揭示了四环、内部凸起以及下部茎干中的AGC三联体中的镁离子结合位点。我们的结果表明,四环、凸起和三联体区域内的结构、静电环境以及镁离子结合位点是II类内含子和剪接体剪接机制的保守特征,可能是催化功能的关键。

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