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一种与丛毛单胞菌属菌株CNB-1降解氯硝基苯和硝基苯有关的新型脱氨酶。

A novel deaminase involved in chloronitrobenzene and nitrobenzene degradation with Comamonas sp. strain CNB-1.

作者信息

Liu Lei, Wu Jian-Feng, Ma Ying-Fei, Wang Sheng-Yue, Zhao Guo-Ping, Liu Shuang-Jiang

机构信息

Institute of Microbiology, Chinese Academy of Sciences, ZhongGuanCun, Haidian, Beijing 100080, People's Republic of China.

出版信息

J Bacteriol. 2007 Apr;189(7):2677-82. doi: 10.1128/JB.01762-06. Epub 2007 Jan 26.

Abstract

Comamonas sp. strain CNB-1 degrades nitrobenzene and chloronitrobenzene via the intermediates 2-aminomuconate and 2-amino-5-chloromuconate, respectively. Deamination of these two compounds results in the release of ammonia, which is used as a source of nitrogen for bacterial growth. In this study, a novel deaminase was purified from Comamonas strain CNB-1, and the gene (cnbZ) encoding this enzyme was cloned. The N-terminal sequence and peptide fingerprints of this deaminase were determined, and BLAST searches revealed no match with significant similarity to any functionally characterized proteins. The purified deaminase is a monomer (30 kDa), and its V(max) values for 2-aminomuconate and 2-amino-5-chloromuconate were 147 micromol x min(-1) x mg(-1) and 196 micromol x min(-1) x mg(-1), respectively. Its catalytic products from 2-aminomuconate and 2-amino-5-chloromuconate were 2-hydroxymuconate and 2-hydroxy-5-chloromuconate, respectively, which are different from those previously reported for the deaminases of Pseudomonas species. In the catalytic mechanism proposed, the alpha-carbon and nitrogen atoms (of both 2-aminomuconate and 2-amino-5-chloromuconate) were simultaneously attacked by a hydroxyl group and a proton, respectively. Homologs of cnbZ were identified in the genomes of Bradyrhizobium japonicum, Rhodopseudomonas palustris, and Roseiflexus sp. strain RS-1; these genes were previously annotated as encoding hypothetical proteins of unknown function. It is concluded that CnbZ represents a novel enzyme that deaminates xenobiotic compounds and/or alpha-amino acids.

摘要

食酸菌属菌株CNB-1分别通过中间体2-氨基粘康酸和2-氨基-5-氯粘康酸降解硝基苯和氯硝基苯。这两种化合物的脱氨基作用导致氨的释放,氨被用作细菌生长的氮源。在本研究中,从食酸菌菌株CNB-1中纯化出一种新型脱氨酶,并克隆了编码该酶的基因(cnbZ)。测定了该脱氨酶的N端序列和肽指纹图谱,通过BLAST搜索发现,与任何功能已明确的蛋白质均无显著相似性匹配。纯化后的脱氨酶为单体(30 kDa),其对2-氨基粘康酸和2-氨基-5-氯粘康酸的Vmax值分别为147 μmol·min-1·mg-1和196 μmol·min-1·mg-1。其催化2-氨基粘康酸和2-氨基-5-氯粘康酸的产物分别为2-羟基粘康酸和2-羟基-5-氯粘康酸,这与先前报道的假单胞菌属脱氨酶的产物不同。在所提出的催化机制中,(2-氨基粘康酸和2-氨基-5-氯粘康酸的)α-碳原子和氮原子分别同时受到一个羟基和一个质子的攻击。在日本慢生根瘤菌、沼泽红假单胞菌和红弯菌属菌株RS-1的基因组中鉴定出了cnbZ的同源物;这些基因先前被注释为编码功能未知的假定蛋白质。得出的结论是,CnbZ代表一种可使外源化合物和/或α-氨基酸脱氨基的新型酶。

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