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苯磷酸合酶:一种催化芳香陶厄氏菌厌氧苯酚代谢第一步的新型磷酸转移酶。

Phenylphosphate synthase: a new phosphotransferase catalyzing the first step in anaerobic phenol metabolism in Thauera aromatica.

作者信息

Schmeling Sirko, Narmandakh Ariun, Schmitt Oliver, Gad'on Nasser, Schühle Karola, Fuchs Georg

机构信息

Institut Biologie II, Mikrobiologie, Albert-Ludwigs-Universität Freiburg, D-79104 Freiburg, Germany.

出版信息

J Bacteriol. 2004 Dec;186(23):8044-57. doi: 10.1128/JB.186.23.8044-8057.2004.

Abstract

The anaerobic metabolism of phenol in the beta-proteobacterium Thauera aromatica proceeds via para-carboxylation of phenol (biological Kolbe-Schmitt carboxylation). In the first step, phenol is converted to phenylphosphate which is then carboxylated to 4-hydroxybenzoate in the second step. Phenylphosphate formation is catalyzed by the novel enzyme phenylphosphate synthase, which was studied. Phenylphosphate synthase consists of three proteins whose genes are located adjacent to each other on the phenol operon and were overproduced in Escherichia coli. The promoter region and operon structure of the phenol gene cluster were investigated. Protein 1 (70 kDa) resembles the central part of classical phosphoenolpyruvate synthase which contains a conserved histidine residue. It catalyzes the exchange of free [(14)C]phenol and the phenol moiety of phenylphosphate but not the phosphorylation of phenol. Phosphorylation of phenol requires protein 1, MgATP, and another protein, protein 2 (40 kDa), which resembles the N-terminal part of phosphoenol pyruvate synthase. Proteins 1 and 2 catalyze the following reaction: phenol + MgATP + H(2)O-->phenylphosphate + MgAMP + orthophosphate. The phosphoryl group in phenylphosphate is derived from the beta-phosphate group of ATP. The free energy of ATP hydrolysis obviously favors the trapping of phenol (K(m), 0.04 mM), even at a low ambient substrate concentration. The reaction is stimulated severalfold by another protein, protein 3 (24 kDa), which contains two cystathionine-beta-synthase domains of unknown function but does not show significant overall similarity to known proteins. The molecular and catalytic features of phenylphosphate synthase resemble those of phosphoenolpyruvate synthase, albeit with interesting modifications.

摘要

β-变形菌属嗜芳烃陶厄氏菌中苯酚的厌氧代谢通过苯酚的对羧化作用(生物科尔贝-施密特羧化反应)进行。第一步,苯酚转化为苯基磷酸酯,然后在第二步中羧化为4-羟基苯甲酸。苯基磷酸酯的形成由新型酶苯基磷酸酯合酶催化,该酶已被研究。苯基磷酸酯合酶由三种蛋白质组成,其基因在苯酚操纵子上彼此相邻定位,并在大肠杆菌中过量表达。对苯酚基因簇的启动子区域和操纵子结构进行了研究。蛋白质1(70 kDa)类似于经典磷酸烯醇丙酮酸合酶的中心部分,其中含有一个保守的组氨酸残基。它催化游离的[¹⁴C]苯酚与苯基磷酸酯的苯酚部分之间的交换,但不催化苯酚的磷酸化。苯酚的磷酸化需要蛋白质1、MgATP和另一种蛋白质,即蛋白质2(40 kDa),它类似于磷酸烯醇丙酮酸合酶的N端部分。蛋白质1和蛋白质2催化以下反应:苯酚 + MgATP + H₂O→苯基磷酸酯 + MgAMP + 正磷酸盐。苯基磷酸酯中的磷酰基来自ATP的β-磷酸基团。即使在低环境底物浓度下,ATP水解的自由能显然有利于捕获苯酚(Kₘ,0.04 mM)。该反应受到另一种蛋白质,即蛋白质3(24 kDa)的刺激,其倍数增加,蛋白质3含有两个功能未知的胱硫醚-β-合酶结构域,但与已知蛋白质没有明显的整体相似性。苯基磷酸酯合酶的分子和催化特征类似于磷酸烯醇丙酮酸合酶,尽管有有趣的修饰。

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