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真菌芳基醇氧化酶晶体结构揭示的氧化还原酶GMC家族中的新结构特征。

Novel structural features in the GMC family of oxidoreductases revealed by the crystal structure of fungal aryl-alcohol oxidase.

作者信息

Fernández Israel S, Ruíz-Dueñas Francisco J, Santillana Elena, Ferreira Patricia, Martínez María Jesús, Martínez Angel T, Romero Antonio

机构信息

Centro de Investigaciones Biológicas, CSIC, E-28040 Madrid, Spain.

出版信息

Acta Crystallogr D Biol Crystallogr. 2009 Nov;65(Pt 11):1196-205. doi: 10.1107/S0907444909035860. Epub 2009 Oct 22.

DOI:10.1107/S0907444909035860
PMID:19923715
Abstract

Lignin biodegradation, a key step in carbon recycling in land ecosystems, is carried out by white-rot fungi through an H(2)O(2)-dependent process defined as enzymatic combustion. Pleurotus eryngii is a selective lignin-degrading fungus that produces H(2)O(2) during redox cycling of p-anisylic compounds involving the secreted flavoenzyme aryl-alcohol oxidase (AAO). Here, the 2.4 A resolution X-ray crystal structure of this oxidoreductase, which catalyzes dehydrogenation reactions on various primary polyunsaturated alcohols, yielding the corresponding aldehydes, is reported. The AAO crystal structure was solved by single-wavelength anomalous diffraction of a selenomethionine derivative obtained by Escherichia coli expression and in vitro folding. This monomeric enzyme is composed of two domains, the overall folding of which places it into the GMC (glucose-methanol-choline oxidase) oxidoreductase family, and a noncovalently bound FAD cofactor. However, two additional structural elements exist in the surroundings of its active site that modulate the access of substrates; these are absent in the structure of the model GMC oxidoreductase glucose oxidase. The folding of these novel elements gives rise to a funnel-like hydrophobic channel that connects the solvent region to the buried active-site cavity of AAO. This putative active-site cavity is located in front of the re side of the FAD isoalloxazine ring and near two histidines (His502 and His546) that could contribute to alcohol activation as catalytic bases. Moreover, three aromatic side chains from two phenylalanines (Phe397 and Phe502) and one tyrosine (Tyr92) at the inner region of the channel form an aromatic gate that may regulate the access of the enzyme substrates to the active site as well as contribute to the recognition of the alcohols that can effectively be oxidized by AAO.

摘要

木质素生物降解是陆地生态系统中碳循环的关键步骤,由白腐真菌通过一种依赖H₂O₂的过程进行,该过程被定义为酶促燃烧。杏鲍菇是一种选择性木质素降解真菌,在对甲氧基苯甲酸化合物的氧化还原循环过程中,通过分泌的黄素酶芳基醇氧化酶(AAO)产生H₂O₂。在此,报道了这种氧化还原酶的2.4埃分辨率X射线晶体结构,该酶催化各种伯多不饱和醇的脱氢反应,生成相应的醛。通过大肠杆菌表达和体外折叠获得的硒代蛋氨酸衍生物的单波长反常衍射解析了AAO晶体结构。这种单体酶由两个结构域组成,其整体折叠使其属于GMC(葡萄糖 - 甲醇 - 胆碱氧化酶)氧化还原酶家族,并含有一个非共价结合的FAD辅因子。然而,在其活性位点周围存在另外两个调节底物进入的结构元件;这些在模型GMC氧化还原酶葡萄糖氧化酶的结构中不存在。这些新元件的折叠产生了一个漏斗状的疏水通道,将溶剂区域连接到AAO的埋藏活性位点腔。这个假定的活性位点腔位于FAD异咯嗪环的Re侧前方,靠近两个可能作为催化碱基促进醇活化的组氨酸(His502和His546)。此外,通道内部区域的两个苯丙氨酸(Phe397和Phe502)和一个酪氨酸(Tyr92)的三个芳香族侧链形成一个芳香门,可能调节酶底物进入活性位点,并有助于识别可被AAO有效氧化的醇。

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