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来自牛蛙(美国牛蛙)卵母细胞的一种细胞毒性核糖核酸酶的溶液结构。

The solution structure of a cytotoxic ribonuclease from the oocytes of Rana catesbeiana (bullfrog).

作者信息

Chang C F, Chen C, Chen Y C, Hom K, Huang R F, Huang T H

机构信息

Institute of Biomedical Sciences, Academia Sinica, Nankang, Taipei, Taiwan, 11529, The Republic of China.

出版信息

J Mol Biol. 1998;283(1):231-44. doi: 10.1006/jmbi.1998.2082.

DOI:10.1006/jmbi.1998.2082
PMID:9761686
Abstract

RC-RNase is a pyrimidine-guanine sequence-specific ribonuclease and a lectin possessing potent cell cytotoxicity. It was isolated from the oocytes of Rana catesbeiana (bull frog). From analysis of an extensive set of 1H homonuclear 2D NMR spectra we have completed the resonance assignments. Determination of the three-dimensional structure was carried out with the program X-PLOR using a total of 951 restraints including 814 NMR-derived distances, 61 torsion angles, and 76 hydrogen bond restraints. In the resultant family of 15 best structures, selected from a total of 150 calculated structures, the root-mean-square deviation from the average structure for the backbone heavy-atoms involved in well-defined secondary structure is 0.48 A, while that for all backbone heavy-atoms is 0.91 A. The structure of RC-RNase consists of three alpha-helices and two triple-stranded anti-parallel beta-sheets and folds in a kidney-shape, very similar to the X-ray crystal structure of a homolo gous protein, onconase isolated from Rana pipiens. We have also investigated the interaction between RC-RNase and two inhibitors, cytidylyl(2'-->5')guanosine (2',5'-CpG) and 2'-deoxycytidylyl(3'-->5')-2'-deoxyguanosine (3',5'-dCpdG). Based on the ligand-induced chemical shift changes in RC-RNase and the NOE cross-peaks between RC-RNase and the inhibitors, the key residues involved in protein-inhibitor interaction have been identified. The inhibitors were found to bind in a "retro-binding" mode, with the guanine base bonded to the B1 subsite. The His103 residue was found to occupy the B state with the imidazole ring pointing away from the active site. The structure coordinates and the NMR restraints have been deposited in the Brookhaven Protein Data Bank (1bc4 and 1bc4mr, respectively).

摘要

RC核糖核酸酶是一种嘧啶 - 鸟嘌呤序列特异性核糖核酸酶,也是一种具有强大细胞毒性的凝集素。它是从牛蛙(Rana catesbeiana)的卵母细胞中分离出来的。通过对大量的1H同核二维核磁共振谱进行分析,我们完成了共振归属。使用X-PLOR程序确定三维结构,总共使用了951个约束条件,包括814个源自核磁共振的距离、61个扭转角和76个氢键约束。在从总共150个计算结构中选出的15个最佳结构家族中,参与明确二级结构的主链重原子相对于平均结构的均方根偏差为0.48埃,而所有主链重原子的均方根偏差为0.91埃。RC核糖核酸酶的结构由三个α螺旋和两个三链反平行β折叠组成,呈肾形折叠,与从豹蛙(Rana pipiens)分离出的同源蛋白癌蛙酶的X射线晶体结构非常相似。我们还研究了RC核糖核酸酶与两种抑制剂,即胞苷酰(2'→5')鸟苷(2',5'-CpG)和2'-脱氧胞苷酰(3'→5')-2'-脱氧鸟苷(3',5'-dCpdG)之间的相互作用。基于RC核糖核酸酶中配体诱导的化学位移变化以及RC核糖核酸酶与抑制剂之间的核Overhauser效应交叉峰,确定了参与蛋白质 - 抑制剂相互作用的关键残基。发现抑制剂以“反向结合”模式结合,鸟嘌呤碱基与B1亚位点结合。发现His103残基处于B状态,咪唑环指向远离活性位点的方向。结构坐标和核磁共振约束条件已分别存入布鲁克海文蛋白质数据库(分别为1bc4和1bc4mr)。

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