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噬菌体φ29原头部RNA-连接体相互作用的丙氨酸扫描和Fe-BABE探测

Alanine scanning and Fe-BABE probing of the bacteriophage ø29 prohead RNA-connector interaction.

作者信息

Atz Rockney, Ma Shuhua, Gao Jiali, Anderson Dwight L, Grimes Shelley

机构信息

Department of Diagnostic and Biological Sciences, University of Minnesota, Minneapolis, MN 55455, USA.

出版信息

J Mol Biol. 2007 May 25;369(1):239-48. doi: 10.1016/j.jmb.2007.03.033. Epub 2007 Mar 20.

Abstract

The DNA packaging motor of the Bacillus subtilis bacteriophage ø29 prohead is comprised in part of an oligomeric ring of 174 base RNA molecules (pRNA) positioned near the N termini of subunits of the dodecameric head-tail connector. Deletion and alanine substitution mutants in the connector protein (gp10) N terminus were assembled into proheads in Escherichia coli and the particles tested for pRNA binding and DNA-gp3 packaging in vitro. The basic amino acid residues RKR at positions 3-5 of the gp10 N terminus were central to pRNA binding during assembly of an active DNA packaging motor. Conjugation of iron(S)-1-(p-bromoacetamidobenzyl) ethylenediaminetetraacetate (Fe-BABE) to residue S170C in the narrow end of the connector, near the N terminus, permitted hydroxyl radical probing of bound [(32)P]pRNA and identified two discrete sites proximal to this residue: the C-helix at the junction of the A, C and D helices, and the E helix and the CE loop/D loop of the intermolecular base pairing site.

摘要

枯草芽孢杆菌噬菌体ø29原头部的DNA包装马达部分由174个碱基的RNA分子(pRNA)的寡聚环组成,该寡聚环位于十二聚体头尾连接体亚基的N端附近。将连接蛋白(gp10)N端的缺失和丙氨酸替代突变体在大肠杆菌中组装成原头部,并对这些颗粒进行体外pRNA结合和DNA-gp3包装测试。gp10 N端第3至5位的碱性氨基酸残基RKR在活性DNA包装马达组装过程中对pRNA结合至关重要。将铁(S)-1-(对溴乙酰氨基苄基)乙二胺四乙酸(Fe-BABE)与连接体窄端靠近N端的S170C残基偶联,可对结合的[(32)P]pRNA进行羟基自由基探测,并确定该残基附近的两个离散位点:A、C和D螺旋交界处的C螺旋,以及分子间碱基配对位点的E螺旋和CE环/D环。

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