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p-cresol methylhydroxylase from a denitrifying bacterium involved in anaerobic degradation of p-cresol.

机译:来自反硝化细菌的对甲酚甲基羟化酶,涉及对甲酚的厌氧降解。

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摘要

A bacterium, strain PC-07, previously isolated as part of a coculture capable of growing on p-cresol under anaerobic conditions with nitrate as the acceptor was identified as an Achromobacter sp. The first enzyme of the pathway, p-cresol methylhydroxylase, which converts its substrate into p-hydroxybenzyl alcohol, was purified. The enzyme had an Mr of 130,000 and the spectrum of a flavocytochrome. It was composed of flavoprotein subunits of Mr 54,000 and cytochrome subunits of Mr 12,500. The midpoint redox potential of the cytochrome was 232 mV. The Km and kcat for p-cresol were 21 microM and 112 s-1 respectively, and the Km for phenazine methosulfate, the artificial acceptor used in the assays, was determined to be 1.7 mM. These properties place the enzyme in the same class as the p-cresol methylhydroxylases from aerobically isolated Pseudomonas spp.
机译:先前作为共培养物的一部分分离出的细菌PC-07菌株被鉴定为无色杆菌属,该细菌能够在厌氧条件下在对甲酚中以硝酸盐为受体在共甲酚中生长。纯化了该途径的第一个酶,即对甲酚甲基羟化酶,该酶将其底物转化为对羟基苄醇。该酶的Mr为130,000,黄素细胞色素的光谱。它由54,000先生的黄素蛋白亚基和12,500先生的细胞色素亚基组成。细胞色素的中点氧化还原电位为232 mV。对甲酚的Km和kcat分别为21 microM和112 s-1,测定中使用的人工受体吩甲基硫酸甲酯的Km为1.7 mM。这些特性使该酶与需氧分离的假单胞菌属(Pseudomonas spp)的对甲酚甲基羟基酶同属一类。

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