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从亚硫酸磺杆菌中纯化和表征二甲基硫醚单加氧酶。

Purification and characterization of dimethylsulfide monooxygenase from Hyphomicrobium sulfonivorans.

机构信息

School of Life Sciences, University of Warwick, Wellesbourne, UK.

出版信息

J Bacteriol. 2011 Mar;193(5):1250-8. doi: 10.1128/JB.00977-10. Epub 2011 Jan 7.

Abstract

Dimethylsulfide (DMS) is a volatile organosulfur compound which has been implicated in the biogeochemical cycling of sulfur and in climate control. Microbial degradation is a major sink for DMS. DMS metabolism in some bacteria involves its oxidation by a DMS monooxygenase in the first step of the degradation pathway; however, this enzyme has remained uncharacterized until now. We have purified a DMS monooxygenase from Hyphomicrobium sulfonivorans, which was previously isolated from garden soil. The enzyme is a member of the flavin-linked monooxygenases of the luciferase family and is most closely related to nitrilotriacetate monooxygenases. It consists of two subunits: DmoA, a 53-kDa FMNH₂-dependent monooxygenase, and DmoB, a 19-kDa NAD(P)H-dependent flavin oxidoreductase. Enzyme kinetics were investigated with a range of substrates and inhibitors. The enzyme had a K(m) of 17.2 (± 0.48) μM for DMS (k(cat) = 5.45 s⁻¹) and a V(max) of 1.25 (± 0.01) μmol NADH oxidized min⁻¹ (mg protein⁻¹). It was inhibited by umbelliferone, 8-anilinonaphthalenesulfonate, a range of metal-chelating agents, and Hg²(+), Cd²(+), and Pb²(+) ions. The purified enzyme had no activity with the substrates of related enzymes, including alkanesulfonates, aldehydes, nitrilotriacetate, or dibenzothiophenesulfone. The gene encoding the 53-kDa enzyme subunit has been cloned and matched to the enzyme subunit by mass spectrometry. DMS monooxygenase represents a new class of FMNH₂-dependent monooxygenases, based on its specificity for dimethylsulfide and the molecular phylogeny of its predicted amino acid sequence. The gene encoding the large subunit of DMS monooxygenase is colocated with genes encoding putative flavin reductases, homologues of enzymes of inorganic and organic sulfur compound metabolism, and enzymes involved in riboflavin synthesis.

摘要

二甲基硫(DMS)是一种挥发性有机硫化合物,它与硫的生物地球化学循环和气候控制有关。微生物降解是 DMS 的主要汇。在一些细菌中,DMS 的代谢涉及 DMS 单加氧酶在降解途径的第一步中氧化;然而,直到现在,这种酶仍然没有被描述。我们从先前从花园土壤中分离出的硫杆菌属中纯化了一种 DMS 单加氧酶。该酶是荧光素连接的单加氧酶家族中的一员,与三聚氰胺单加氧酶最为密切相关。它由两个亚基组成:DmoA,一种 53kDa 的 FMNH₂ 依赖性单加氧酶,和 DmoB,一种 19kDa 的 NAD(P)H 依赖性黄素氧化还原酶。用一系列的底物和抑制剂研究了酶的动力学。该酶对 DMS 的 K(m)为 17.2(±0.48)μM(k(cat)=5.45s⁻¹),V(max)为 1.25(±0.01)μmol NADH 氧化 min⁻¹(mg 蛋白⁻¹)。它被 Umbelliferone、8-苯胺萘磺酸盐、一系列金属螯合剂以及 Hg²(+)、Cd²(+)和 Pb²(+)离子抑制。纯化的酶对烷基亚磺酸盐、醛、三聚氰胺或二苯并噻吩砜等相关酶的底物没有活性。编码 53kDa 酶亚基的基因已经被克隆,并通过质谱与酶亚基相匹配。DMS 单加氧酶代表了一类新的 FMNH₂ 依赖性单加氧酶,基于其对二甲基硫的特异性和其预测氨基酸序列的分子系统发育。DMS 单加氧酶大亚基的基因与编码黄素还原酶的基因、无机和有机硫化合物代谢酶的同源物以及参与核黄素合成的酶一起定位于基因座上。

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