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嗜热栖热菌核糖核酸酶P蛋白的核磁共振共振归属

NMR resonance assignments of RNase P protein from Thermotoga maritima.

作者信息

Zeng Danyun, Brown Benjamin P, Voehler Markus W, Cai Sheng, Reiter Nicholas J

机构信息

Department of Chemistry, Marquette University, Milwaukee, WI, USA.

Chemical and Physical Biology Program, Vanderbilt University, Nashville, TN, USA.

出版信息

Biomol NMR Assign. 2018 Apr;12(1):183-187. doi: 10.1007/s12104-018-9806-7. Epub 2018 Feb 15.

Abstract

Ribonuclase P (RNase P) is an essential metallo-endonuclease that catalyzes 5' precursor-tRNA (ptRNA) processing and exists as an RNA-based enzyme in bacteria, archaea, and eukaryotes. In bacteria, a large catalytic RNA and a small protein component assemble to recognize and accurately cleave ptRNA and tRNA-like molecular scaffolds. Substrate recognition of ptRNA by bacterial RNase P requires RNA-RNA shape complementarity, intermolecular base pairing, and a dynamic protein-ptRNA binding interface. To gain insight into the binding specificity and dynamics of the bacterial protein-ptRNA interface, we report the backbone and side chain H, C, and N resonance assignments of the hyperthermophilic Thermatoga maritima RNase P protein in solution at 318 K. Our data confirm the formation of a stable RNA recognition motif (RRM) with intrinsic heterogeneity at both the N- and C-terminus of the protein, consistent with available structural information. Comprehensive resonance assignments of the bacterial RNase P protein serve as an important first step in understanding how coupled RNA binding and protein-RNA conformational changes give rise to ribonucleoprotein function.

摘要

核糖核酸酶P(RNase P)是一种必需的金属内切核酸酶,可催化5'前体tRNA(ptRNA)的加工,在细菌、古细菌和真核生物中以一种基于RNA的酶形式存在。在细菌中,一个大的催化RNA和一个小的蛋白质组分组装在一起,以识别并准确切割ptRNA和tRNA样分子支架。细菌RNase P对ptRNA的底物识别需要RNA-RNA形状互补、分子间碱基配对以及一个动态的蛋白质-ptRNA结合界面。为了深入了解细菌蛋白质-ptRNA界面的结合特异性和动力学,我们报道了嗜热栖热菌RNase P蛋白在318 K溶液中的主链和侧链H、C和N共振归属。我们的数据证实了该蛋白质在N端和C端均形成了具有内在异质性的稳定RNA识别基序(RRM),这与现有的结构信息一致。细菌RNase P蛋白的全面共振归属是理解RNA结合与蛋白质-RNA构象变化如何共同产生核糖核蛋白功能的重要第一步。

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