首页> 美国卫生研究院文献>Journal of Bacteriology >Carboxylation of phenylphosphate by phenol carboxylase an enzyme system of anaerobic phenol metabolism.
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Carboxylation of phenylphosphate by phenol carboxylase an enzyme system of anaerobic phenol metabolism.

机译:苯酚羧化酶(一种厌氧酚代谢的酶系统)将磷酸苯酯羧化。

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摘要

Several lines of evidence indicate that the first step in the anaerobic metabolism of phenol is phenol carboxylation to 4-hydroxybenzoate; this reaction is considered a biological Kolbe-Schmitt carboxylation. A phenol carboxylase system was characterized by using a denitrifying Pseudomonas strain, K 172, which catalyzes an isotope exchange between 14CO2 and the carboxyl group of 4-hydroxybenzoate. The enzymatic isotope exchange activity (100 nmol min-1 mg-1 of protein) requires Mn2+ and K+. We show that this system also catalyzes the carboxylation of phenylphosphate (the phosphoric acid monophenyl ester) to 4-hydroxybenzoate and phosphate. The specific activity of phenylphosphate carboxylation at the optimal pH of 6.5 is 12 nmol of CO2 fixed min-1 mg-1 of protein. Phenylphosphate cannot be replaced by Mg(2+)-ATP and phenol. The carboxylase activity requires Mn2+ but, in contrast to the isotope exchange activity, does not require K+. The apparent Km values are 1.5 mM dissolved CO2 and 0.2 mM phenylphosphate. Several convenient assays for phenylophosphate carboxylation are described. The isotope exchange reaction and the net carboxylation reaction are catalyzed by the same oxygen-sensitive enzyme, which has a half-life in an air-saturated solution of less than 1 min. Both activities cochromatographed with a protein with a Mr of 280,000, and both activities were induced only after anaerobic growth on phenol. The carboxylation of phenylphosphate suggests that phenylphosphate itself is the physiological CO2 acceptor molecular of this novel CO2 fixation reaction. Alternatively, phenylphosphate could simulate the unknown natural precursor. It is suggested that the formation of an enzyme-bound phenolate anion from the activated phenolic compound is the rate-determining step in the carboxylation reaction.
机译:几条证据表明,苯酚厌氧代谢的第一步是将苯酚羧化为4-羟基苯甲酸酯。该反应被认为是生物学的Kolbe-Schmitt羧化反应。酚羧化酶系统的特征是使用反硝化假单胞菌菌株K 172,该菌株催化14CO2与4-羟基苯甲酸酯的羧基之间的同位素交换。酶的同位素交换活性(100 nmol min-1 mg-1的蛋白质)需要Mn2 +和K +。我们表明,该系统还催化苯基磷酸酯(磷酸单苯酯)的羧基化,生成4-羟基苯甲酸酯和磷酸酯。在最佳pH值为6.5时,磷酸磷酸苯酯的比活度为12 nmol的固定CO2 min-1 mg-1蛋白。磷酸苯酯不能用Mg(2 +)-ATP和苯酚代替。羧化酶活性需要Mn2 +,但是与同位素交换活性相反,它不需要K +。表观Km值为1.5 mM溶解的CO2和0.2 mM磷酸苯酯。描述了几种方便的苯磷酸盐磷酸化的测定方法。同位素交换反应和净羧化反应由相同的氧敏感酶催化,该酶在空气饱和溶液中的半衰期少于1分钟。两种活性均用分子量为280,000的蛋白质进行了色谱分离,并且两种活性仅在苯酚上厌氧生长后才被诱导。磷酸苯酯的羧化表明磷酸苯酯本身是这种新颖的二氧化碳固定反应的生理二氧化碳受体分子。或者,磷酸苯酯可以模拟未知的天然前体。建议由活化的酚类化合物形成酶结合的酚酸根阴离子是羧化反应中决定速率的步骤。

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