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嗜热脂肪芽孢杆菌含小Toprim结构域蛋白的晶体结构及假定功能

Crystal structure and putative function of small Toprim domain-containing protein from Bacillus stearothermophilus.

作者信息

Rezácová Pavlína, Borek Dominika, Moy Shiu F, Joachimiak Andrzej, Otwinowski Zbyszek

机构信息

Department of Biochemistry, UT Southwestern Medical Center, Dallas, Texas 75390-8816, USA.

出版信息

Proteins. 2008 Feb 1;70(2):311-9. doi: 10.1002/prot.21511.

Abstract

The crystal structure of the Midwest Center for Structural Genomics target APC35832, a 14.7-kDa cytosolic protein from Bacillus stearothermophilus, has been determined at 1.3 A resolution by the single anomalous diffraction method from a mercury soaked crystal. The APC35832 protein is a representative of large group of bacterial and archeal proteins entirely consisting of the Toprim (topoisomerase-primase) domain. This domain is found in the catalytic centers of many enzymes catalyzing phosphodiester bond formation or cleavage, but the function of small Toprim domain proteins remains unknown. Consistent with the sequence analysis, the APC35832 structure shows a conserved Toprim fold, with a central 4-stranded parallel beta-sheet surrounded by four alpha-helixes. Comparison of the APC35832 structure with its closest structural homolog, the catalytic core of bacteriophage T7 primase, revealed structural conservation of a metal binding site and isothermal titration calorimetry indicates that APC35832 binds Mg2+ with a sub-millimolar dissociation constant (K(d)). The APC35832-Mg2+ complex structure was determined at 1.65 A and reveals the role of conserved acidic residues in Mg2+ ion coordination. The structural similarities to other Toprim domain containing proteins and potential function and substrates of APC35832 are discussed in this article.

摘要

中西部结构基因组学中心的目标蛋白APC35832是一种来自嗜热脂肪芽孢杆菌的14.7 kDa胞质蛋白,通过对汞浸泡晶体采用单波长反常衍射法,已在1.3 Å分辨率下测定了其晶体结构。APC35832蛋白是一大类完全由Toprim(拓扑异构酶-引发酶)结构域组成的细菌和古细菌蛋白的代表。该结构域存在于许多催化磷酸二酯键形成或断裂的酶的催化中心,但小型Toprim结构域蛋白的功能仍不清楚。与序列分析一致,APC35832的结构显示出保守的Toprim折叠,中央有一个由四条α螺旋包围的四链平行β折叠。将APC35832的结构与其最接近的结构同源物噬菌体T7引发酶的催化核心进行比较,发现了一个金属结合位点的结构保守性,等温滴定量热法表明APC用亚毫摩尔解离常数(Kd)结合Mg2+。APC35832-Mg2+复合物的结构在1.65 Å分辨率下测定,揭示了保守酸性残基在Mg2+离子配位中的作用。本文讨论了与其他含Toprim结构域蛋白的结构相似性以及APC35832的潜在功能和底物。

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