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大肠杆菌16S rRNA中核糖体蛋白S8结合位点的核磁共振结构测定。

NMR structure determination of the binding site for ribosomal protein S8 from Escherichia coli 16 S rRNA.

作者信息

Kalurachchi K, Nikonowicz E P

机构信息

Department of Biochemistry and Cell Biology, Rice University, Houston, TX 77005, USA.

出版信息

J Mol Biol. 1998 Jul 24;280(4):639-54. doi: 10.1006/jmbi.1998.1915.

DOI:10.1006/jmbi.1998.1915
PMID:9677294
Abstract

Many cellular processes involve the preferential interaction of an RNA molecule with a specific protein. A detailed analysis of the individual protein and RNA components of these interactions can provide unique insights into the structural features important for protein-RNA recognition. Ribosomal protein S8 of Escherichia coli plays a key role in 30 S ribosomal subunit assembly through its interaction with 16 S rRNA. The binding site for protein S8 comprises a portion of helix 21, nucleotides G588 to G604 and C634 to C651. This region forms a base-paired helix that is interrupted by a non-Watson-Crick segment composed of nine phylogenetically conserved nucleotides. We have investigated the detailed structure of the conserved segment and the interaction of this region with metal ions using NMR spectroscopy. Twenty-four of the 40 calculated structures converged to similar conformations and were grouped into two families. The main difference between the families is the orientation of the base of U641. The rms deviation between the heavy-atoms of the ten lowest-energy structures is 1.24 A. The orientations of the G597.C643 base-pair and A595.(A596.U644) base-triple within the conserved core have been defined and appear to extend the proximal segment of helix 21 into the phylogenetically conserved core. The base of A642 terminates this helix by stacking against C643 and the base of U641 forms hydrogen bonds with core nucleotides. The conserved core also contains a Mg2+-binding site that promotes stabilization of the secondary and tertiary structure elements of the core. A model for the interaction of S8 with its RNA-binding site is proposed.

摘要

许多细胞过程都涉及RNA分子与特定蛋白质的优先相互作用。对这些相互作用中单个蛋白质和RNA成分进行详细分析,可为蛋白质-RNA识别的重要结构特征提供独特见解。大肠杆菌的核糖体蛋白S8通过与16S rRNA相互作用,在30S核糖体亚基组装中起关键作用。蛋白质S8的结合位点包括螺旋21的一部分,核苷酸G588至G604以及C634至C651。该区域形成一个碱基配对螺旋,被由九个系统发育保守核苷酸组成的非沃森-克里克片段打断。我们使用核磁共振光谱研究了保守片段的详细结构以及该区域与金属离子的相互作用。计算出的40个结构中有24个收敛到相似构象,并分为两个家族。两个家族之间的主要区别在于U641碱基的方向。十个最低能量结构的重原子之间的均方根偏差为1.24埃。已确定保守核心内G597·C643碱基对和A595·(A596·U644)碱基三联体的方向,它们似乎将螺旋21的近端片段延伸到系统发育保守核心中。A642的碱基通过与C643堆积终止该螺旋,U641的碱基与核心核苷酸形成氢键。保守核心还包含一个Mg2+结合位点,可促进核心二级和三级结构元件的稳定。提出了S8与其RNA结合位点相互作用的模型。

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