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卡那霉素核苷酸转移酶的分子结构解析至3.0埃分辨率。

Molecular structure of kanamycin nucleotidyltransferase determined to 3.0-A resolution.

作者信息

Sakon J, Liao H H, Kanikula A M, Benning M M, Rayment I, Holden H M

机构信息

Institute for Enzyme Research, Graduate School, University of Wisconsin, Madison 53705.

出版信息

Biochemistry. 1993 Nov 16;32(45):11977-84. doi: 10.1021/bi00096a006.

DOI:10.1021/bi00096a006
PMID:8218273
Abstract

Kanamycin nucleotidyltransferase, as originally isolated from Staphylococcus aureus, inactivates the antibiotic kanamycin by catalyzing the transfer of a nucleotidyl group from nucleoside triphosphates such as ATP to the 4'-hydroxyl group of the aminoglycoside. The molecular structure of the enzyme described here was determined by X-ray crystallographic analysis to a resolution of 3.0 A. Crystals employed in the investigation belonged to the space group P4(3)2(1)2 with unit cell dimensions of a = b = 78.9 A and c = 219.2 A. An electron density map phased with seven heavy-atom derivatives revealed that the molecules packed in the crystalline lattice as dimers exhibiting local 2-fold rotation axes. Subsequent symmetry averaging and solvent flattening improved the quality of the electron density such that it was possible to completely trace the 253 amino acid polypeptide chain. Each monomer is divided into two distinct structural domains: the N-terminal motif composed of residues Met 1-Glu 127 and the C-terminal half delineated by residues Ala 128-Phe 253. The N-terminal region is characterized by a five-stranded mixed beta-pleated sheet whereas the C-terminal domain contains five alpha-helices, four of which form an up-and-down alpha-helical bundle very similar to that observed in cytochrome c'. The two subunits wrap about one another to form an ellipsoid with a pronounced cleft that could easily accommodate the various aminoglycosides known to bind to the enzyme.

摘要

卡那霉素核苷酸转移酶最初是从金黄色葡萄球菌中分离出来的,它通过催化核苷三磷酸(如ATP)中的核苷酸基团转移到氨基糖苷的4'-羟基上,使抗生素卡那霉素失活。本文所述酶的分子结构通过X射线晶体学分析确定,分辨率为3.0埃。研究中使用的晶体属于空间群P4(3)2(1)2,晶胞参数为a = b = 78.9埃,c = 219.2埃。用七种重原子衍生物进行相位分析的电子密度图显示,分子在晶格中以二聚体形式堆积,呈现局部二重旋转轴。随后的对称平均和溶剂平整提高了电子密度的质量,从而能够完全追踪253个氨基酸的多肽链。每个单体分为两个不同的结构域:由Met 1-Glu 127残基组成的N端基序和由Ala 128-Phe 253残基界定的C端部分。N端区域的特征是一个五链混合β折叠片层,而C端结构域包含五个α螺旋,其中四个形成一个上下α螺旋束,与细胞色素c'中观察到的非常相似。两个亚基相互缠绕形成一个椭球体,有一个明显的裂缝,很容易容纳已知与该酶结合的各种氨基糖苷。

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