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枯草芽孢杆菌噬菌体SPO1编码的II型DNA结合蛋白TF1在溶液中的结构

Structure of the Bacillus subtilis phage SPO1-encoded type II DNA-binding protein TF1 in solution.

作者信息

Jia X, Grove A, Ivancic M, Hsu V L, Geiduscheck E P, Kearns D R

机构信息

Department of Chemistry and Biochemistry, University of California, San Diego, La Jolla 92093, USA.

出版信息

J Mol Biol. 1996 Oct 25;263(2):259-68. doi: 10.1006/jmbi.1996.0573.

DOI:10.1006/jmbi.1996.0573
PMID:8913305
Abstract

The solution structure of a type II DNA-binding protein, the bacteriophage SPO1-encoded transcription factor 1 (TF1), was determined using NMR spectroscopy. Selective 2H-labeling, 13C-labeling and isotopic heterodimers were used to distinguish contacts between and within monomers of the dimeric protein. A total of 1914 distance and dihedral angle constraints derived from NMR experiments were used in structure calculations using restrained molecular dynamics and simulated annealing protocols. The ensemble of 30 calculated structures has a root-mean-square deviation (r.m.s.d.) of 0.9 A, about the average structure for the backbone atoms, and 1.2 A for all heavy-atoms of the dimeric core (helices 1 and 2) and the beta-sheets. A severe helix distortion at residues 92-93 in the middle of helix 3 is associated with r.m.s.d. of approximately 1.5 A for the helix 3 backbone. Deviations of approximately 5 A or larger are noted for the very flexible beta-ribbon arms that constitute part of a proposed DNA-binding region. A structural model of TF1 has been calculated based on the previously reported crystal structure of the homologous HU protein and this model was used as the starting structure for calculations. A comparison between the calculated average solution structure of TF1 and a solution structure of HU indicates a similarity in the dimeric core (excluding the nine amino acid residue tail) with pairwise deviations of 2 to 3 A. The largest deviations between the average structure and the HU solution structure were found in the beta-ribbon arms, as expected. A 4 A deviation is found at residue 15 of TF1 which is in a loop connecting two helical segments; it has been reported that substitution of Glu15 by Gly increases the thermostability of TF1. The homology between TF1 and other proteins of this family leads us to anticipate similar tertiary structures.

摘要

利用核磁共振光谱法确定了II型DNA结合蛋白噬菌体SPO1编码的转录因子1(TF1)的溶液结构。使用选择性2H标记、13C标记和同位素异源二聚体来区分二聚体蛋白单体之间以及单体内部的接触。在使用受限分子动力学和模拟退火协议进行结构计算时,共使用了1914个源自核磁共振实验的距离和二面角约束。计算得到的30个结构的集合对于主链原子的平均结构,其均方根偏差(r.m.s.d.)为0.9 Å,对于二聚体核心(螺旋1和2)以及β折叠的所有重原子,r.m.s.d.为1.2 Å。螺旋3中部92 - 93位残基处的严重螺旋扭曲与螺旋3主链约1.5 Å的r.m.s.d.相关。对于构成拟议DNA结合区域一部分的非常灵活的β丝带臂,观察到约5 Å或更大的偏差。基于先前报道的同源HU蛋白的晶体结构计算了TF1的结构模型,并将该模型用作计算的起始结构。TF1计算得到的平均溶液结构与HU的溶液结构之间的比较表明,二聚体核心(不包括九个氨基酸残基的尾巴)具有相似性,成对偏差为2至3 Å。正如预期的那样,平均结构与HU溶液结构之间的最大偏差出现在β丝带臂中。在TF1的15位残基处发现了4 Å的偏差,该残基位于连接两个螺旋段的环中;据报道,将Glu15替换为Gly会增加TF1的热稳定性。TF1与该家族其他蛋白质之间的同源性使我们预期它们具有相似的三级结构。

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