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溶液中GDP结合的人c-Ha-Ras蛋白的序列特异性1H和15N共振归属及二级结构

Sequence-specific 1H and 15N resonance assignments and secondary structure of GDP-bound human c-Ha-Ras protein in solution.

作者信息

Muto Y, Yamasaki K, Ito Y, Yajima S, Masaki H, Uozumi T, Wälchli M, Nishimura S, Miyazawa T, Yokoyama S

机构信息

Department of Biophysics and Biochemistry, Faculty of Science, University of Tokyo, Japan.

出版信息

J Biomol NMR. 1993 Mar;3(2):165-84. doi: 10.1007/BF00178260.

DOI:10.1007/BF00178260
PMID:8477185
Abstract

All the backbone 1H and 15N magnetic resonances (except for Pro residues) of the GDP-bound form of a truncated human c-Ha-ras proto-oncogene product (171 amino acid residues, the Ras protein) were assigned by 15N-edited two-dimensional NMR experiments on selectively 15N-labeled Ras proteins in combination with three-dimensional NMR experiments on the uniformly 15N-labeled protein. The sequence-specific assignments were made on the basis of the nuclear Overhauser effect (NOE) connectivities of amide protons with preceding amide and/or C alpha protons. In addition to sequential NOEs, vicinal spin coupling constants for amide protons and C alpha protons and deuterium exchange rates of amide protons were used to characterize the secondary structure of the GDP-bound Ras protein; six beta stands and five helices were identified and the topology of these elements was determined. The secondary structure of the Ras protein in solution was mainly consistent with that in crystal as determined by X-ray analyses. The deuterium exchange rates of amide protons were examined to elucidate the dynamic properties of the secondary structure elements of the Ras protein in solution. In solution, the beta-sheet structure in the Ras protein is rigid, while the second helix (A66-R73) is much more flexible, and the first and fifth helices (S17-124 and V152-L171) are more rigid than other helices. Secondary structure elements at or near the ends of the effector-region loop were found to be much more flexible in solution than in the crystalline state.

摘要

通过对选择性15N标记的Ras蛋白进行15N编辑二维核磁共振实验,并结合对均匀15N标记蛋白进行的三维核磁共振实验,确定了截短的人c-Ha-ras原癌基因产物(171个氨基酸残基,即Ras蛋白)的GDP结合形式的所有主链1H和15N磁共振信号(脯氨酸残基除外)。基于酰胺质子与前一个酰胺和/或Cα质子的核Overhauser效应(NOE)连接性进行了序列特异性归属。除了序列NOE外,还利用酰胺质子和Cα质子的邻位自旋耦合常数以及酰胺质子的氘交换率来表征GDP结合的Ras蛋白的二级结构;确定了6个β链和5个螺旋,并确定了这些元件的拓扑结构。溶液中Ras蛋白的二级结构与X射线分析确定的晶体结构基本一致。通过研究酰胺质子的氘交换率来阐明溶液中Ras蛋白二级结构元件的动态特性。在溶液中,Ras蛋白中的β折叠结构是刚性的,而第二个螺旋(A66-R73)则更加灵活,第一个和第五个螺旋(S17-124和V152-L171)比其他螺旋更刚性。发现在效应器区域环末端或附近的二级结构元件在溶液中比在晶体状态下更加灵活。

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