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泡盛曲霉外切菊粉酶的晶体结构:酶折叠及底物识别的结构决定因素

Crystal structure of exo-inulinase from Aspergillus awamori: the enzyme fold and structural determinants of substrate recognition.

作者信息

Nagem R A P, Rojas A L, Golubev A M, Korneeva O S, Eneyskaya E V, Kulminskaya A A, Neustroev K N, Polikarpov I

机构信息

Instituto de Física de São Carlos, Universidade de São Paulo, Av. Trabalhador São-carlense 400, CEP 13560-970, São Carlos, SP, Brazil.

出版信息

J Mol Biol. 2004 Nov 19;344(2):471-80. doi: 10.1016/j.jmb.2004.09.024.

DOI:10.1016/j.jmb.2004.09.024
PMID:15522299
Abstract

Exo-inulinases hydrolyze terminal, non-reducing 2,1-linked and 2,6-linked beta-d-fructofuranose residues in inulin, levan and sucrose releasing beta-d-fructose. We present the X-ray structure at 1.55A resolution of exo-inulinase from Aspergillus awamori, a member of glycoside hydrolase family 32, solved by single isomorphous replacement with the anomalous scattering method using the heavy-atom sites derived from a quick cryo-soaking technique. The tertiary structure of this enzyme folds into two domains: the N-terminal catalytic domain of an unusual five-bladed beta-propeller fold and the C-terminal domain folded into a beta-sandwich-like structure. Its structural architecture is very similar to that of another member of glycoside hydrolase family 32, invertase (beta-fructosidase) from Thermotoga maritima, determined recently by X-ray crystallography The exo-inulinase is a glycoprotein containing five N-linked oligosaccharides. Two crystal forms obtained under similar crystallization conditions differ by the degree of protein glycosylation. The X-ray structure of the enzyme:fructose complex, at a resolution of 1.87A, reveals two catalytically important residues: Asp41 and Glu241, a nucleophile and a catalytic acid/base, respectively. The distance between the side-chains of these residues is consistent with a double displacement mechanism of reaction. Asp189, which is part of the Arg-Asp-Pro motif, provides hydrogen bonds important for substrate recognition.

摘要

外切菊粉酶可水解菊粉、左聚糖和蔗糖中末端非还原性的2,1-连接和2,6-连接的β-D-呋喃果糖残基,释放出β-D-果糖。我们通过使用源自快速冷冻浸泡技术的重原子位点,采用单对映体置换和反常散射法,解析了泡盛曲霉外切菊粉酶(糖苷水解酶家族32的成员)分辨率为1.55Å的X射线结构。该酶的三级结构折叠成两个结构域:具有不寻常的五叶β-螺旋桨折叠的N端催化结构域和折叠成β-三明治样结构的C端结构域。其结构架构与糖苷水解酶家族32的另一个成员——最近通过X射线晶体学确定结构的嗜热栖热袍菌蔗糖酶(β-果糖苷酶)非常相似。外切菊粉酶是一种含有五个N-连接寡糖的糖蛋白。在相似结晶条件下获得的两种晶体形式在蛋白质糖基化程度上有所不同。该酶与果糖复合物的X射线结构,分辨率为1.87Å,揭示了两个催化重要残基:Asp41和Glu241,分别是亲核试剂和催化酸/碱。这些残基侧链之间的距离与双置换反应机制一致。作为Arg-Asp-Pro基序一部分的Asp189提供了对底物识别很重要的氢键。

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