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氮杂环丁烷-2-羧酸代谢的基因与酶:一种抗生素的解毒与同化作用

Genes and enzymes of azetidine-2-carboxylate metabolism: detoxification and assimilation of an antibiotic.

作者信息

Gross Carol, Felsheim Roderick, Wackett Lawrence P

机构信息

Department of Biochemistry, BioTechnology Institute, 140 Gortner Laboratory, University of Minnesota, St Paul, MN 55108, USA.

出版信息

J Bacteriol. 2008 Jul;190(14):4859-64. doi: 10.1128/JB.02022-07. Epub 2008 May 16.

Abstract

l-(-)-Azetidine-2-carboxylate (AC) is a toxic, natural product analog of l-proline. This study revealed the genes and biochemical strategy employed by Pseudomonas sp. strain A2C to detoxify and assimilate AC as its sole nitrogen source. The gene region from Pseudomonas sp. strain A2C required for detoxification was cloned into Escherichia coli and sequenced. The 7.0-kb region contained eight identifiable genes. Four encoded putative transporters or permeases for gamma-amino acids or drugs. Another gene encoded a homolog of 2-haloacid dehalogenase (HAD). The encoded protein, denoted l-azetidine-2-carboxylate hydrolase (AC hydrolase), was highly overexpressed by subcloning. The AC hydrolase was shown to catalyze azetidine ring opening with the production of 2-hydroxy-4-aminobutyrate. AC hydrolase was further demonstrated to be a new hydrolytic member of the HAD superfamily by showing loss of activity upon changing aspartate-12, the conserved active site nucleophile in this family, to an alanine residue. The presence of a gene encoding a potential export chaperone protein, CsaA, adjacent to the AC hydrolase gene suggested that AC hydrolase might be found inside the periplasm in the native Pseudomonas strain. Periplasmic and cytoplasmic cell fractions from Pseudomonas sp. strain A2C were prepared. A higher specific activity for AC hydrolysis was found in the periplasmic fraction. Protein mass spectrometry further identified AC hydrolase and known periplasmic marker proteins in the periplasmic fraction. A model was proposed in which AC is hydrolyzed in the periplasm and the product of that reaction is transported into and further metabolized in the cytoplasm.

摘要

L-(-)-氮杂环丁烷-2-羧酸(AC)是L-脯氨酸的一种有毒天然产物类似物。本研究揭示了假单胞菌属菌株A2C用于解毒并将AC作为其唯一氮源进行同化的基因和生化策略。将假单胞菌属菌株A2C解毒所需的基因区域克隆到大肠杆菌中并进行测序。这个7.0 kb的区域包含八个可识别的基因。其中四个编码γ-氨基酸或药物的假定转运蛋白或通透酶。另一个基因编码2-卤代酸脱卤酶(HAD)的同源物。所编码的蛋白质,命名为L-氮杂环丁烷-2-羧酸水解酶(AC水解酶),通过亚克隆实现了高度过表达。AC水解酶被证明能催化氮杂环丁烷环开环,生成2-羟基-4-氨基丁酸。通过将天冬氨酸-12(该家族中保守的活性位点亲核试剂)替换为丙氨酸残基后活性丧失,进一步证明AC水解酶是HAD超家族的一个新的水解成员。与AC水解酶基因相邻存在一个编码潜在输出伴侣蛋白CsaA的基因,这表明在天然假单胞菌菌株中AC水解酶可能存在于周质中。制备了假单胞菌属菌株A2C的周质和细胞质细胞组分。在周质组分中发现了对AC水解更高的比活性。蛋白质质谱进一步在周质组分中鉴定出AC水解酶和已知的周质标记蛋白。提出了一个模型,其中AC在周质中被水解,该反应的产物被转运到细胞质中并进一步代谢。

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