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通过对蛋白质进行定点诱变来表征枯草芽孢杆菌PyrR与pyr mRNA的相互作用。

Characterization of the interaction of Bacillus subtilis PyrR with pyr mRNA by site-directed mutagenesis of the protein.

作者信息

Savacool Heather K, Switzer Robert L

机构信息

Department of Biochemistry, University of Illinois, Urbana, Illinois 61801, USA.

出版信息

J Bacteriol. 2002 May;184(9):2521-8. doi: 10.1128/JB.184.9.2521-2528.2002.

DOI:10.1128/JB.184.9.2521-2528.2002
PMID:11948166
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC134998/
Abstract

The Bacillus subtilis PyrR protein regulates transcriptional attenuation of the pyrimidine nucleotide (pyr) operon by binding in a uridine nucleotide-dependent manner to specific sites on pyr mRNA and stabilizing a secondary structure of the downstream RNA that favors termination of transcription. The high-resolution structure of unliganded PyrR was used to guide site-directed mutagenesis of 12 amino acid residues that were thought likely to be involved in the binding of RNA. Missense mutations were constructed and evaluated for their effects on regulation of pyr genes in vivo and their uracil phosphoribosyltransferase activity, which is catalyzed by wild-type PyrR. A substantial fraction of the mutant PyrR proteins did not have native structures, but eight PyrR mutants were purified and characterized physically, for their uracil phosphoribosyltransferase activity and for their ability to bind pyr RNA in vitro. On the basis of these studies Thr-18, His-22, Arg-141, and Arg-146 were implicated in RNA binding. Arg-27 and Lys-152 were also likely to be involved in RNA binding, but Gln substitution mutations in these residues may have altered their subunit-subunit interactions slightly. Arg-19 was implicated in pyr regulation, but a specific role in RNA binding could not be demonstrated because the R19Q mutant protein could not be purified in native form. The results confirm a role in RNA binding of a positively charged face of PyrR previously identified from the crystallographic structure. The RNA binding residues lie in two sequence segments that are conserved in PyrR proteins from many species.

摘要

枯草芽孢杆菌PyrR蛋白通过以尿苷核苷酸依赖的方式结合到pyr mRNA上的特定位点,并稳定下游RNA的二级结构来调节嘧啶核苷酸(pyr)操纵子的转录衰减,该二级结构有利于转录终止。未结合配体的PyrR的高分辨率结构被用于指导对12个氨基酸残基进行定点诱变,这些残基被认为可能参与RNA的结合。构建了错义突变体,并评估了它们对体内pyr基因调控的影响以及它们的尿嘧啶磷酸核糖转移酶活性,该活性由野生型PyrR催化。相当一部分突变的PyrR蛋白没有天然结构,但纯化并物理表征了8个PyrR突变体,检测了它们的尿嘧啶磷酸核糖转移酶活性以及在体外结合pyr RNA的能力。基于这些研究,发现苏氨酸-18、组氨酸-22、精氨酸-141和精氨酸-146参与RNA结合。精氨酸-27和赖氨酸-152也可能参与RNA结合,但这些残基的谷氨酰胺替代突变可能略微改变了它们的亚基-亚基相互作用。精氨酸-19参与pyr调控,但由于R19Q突变蛋白无法以天然形式纯化,因此无法证明其在RNA结合中的具体作用。结果证实了先前从晶体结构中鉴定出的PyrR带正电荷表面在RNA结合中的作用。RNA结合残基位于许多物种的PyrR蛋白中保守的两个序列片段中。

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