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食油假单胞菌1CP对3-氯儿茶酚降解的一种新的改良邻位裂解途径:遗传学和生物化学证据

A new modified ortho cleavage pathway of 3-chlorocatechol degradation by Rhodococcus opacus 1CP: genetic and biochemical evidence.

作者信息

Moiseeva Olga V, Solyanikova Inna P, Kaschabek Stefan R, Gröning Janosch, Thiel Monika, Golovleva Ludmila A, Schlömann Michael

机构信息

Institut für Mikrobiologie, University of Stuttgart, 70550 Stuttgart, Germany.

出版信息

J Bacteriol. 2002 Oct;184(19):5282-92. doi: 10.1128/JB.184.19.5282-5292.2002.

Abstract

The 4-chloro- and 2,4-dichlorophenol-degrading strain Rhodococcus opacus 1CP has previously been shown to acquire, during prolonged adaptation, the ability to mineralize 2-chlorophenol. In addition, homogeneous chlorocatechol 1,2-dioxygenase from 2-chlorophenol-grown biomass has shown relatively high activity towards 3-chlorocatechol. Based on sequences of the N terminus and tryptic peptides of this enzyme, degenerate PCR primers were now designed and used for cloning of the respective gene from genomic DNA of strain 1CP. A 9.5-kb fragment containing nine open reading frames was obtained on pROP1. Besides other genes, a gene cluster consisting of four chlorocatechol catabolic genes was identified. As judged by sequence similarity and correspondence of predicted N termini with those of purified enzymes, the open reading frames correspond to genes for a second chlorocatechol 1,2-dioxygenase (ClcA2), a second chloromuconate cycloisomerase (ClcB2), a second dienelactone hydrolase (ClcD2), and a muconolactone isomerase-related enzyme (ClcF). All enzymes of this new cluster are only distantly related to the known chlorocatechol enzymes and appear to represent new evolutionary lines of these activities. UV overlay spectra as well as high-pressure liquid chromatography analyses confirmed that 2-chloro-cis,cis-muconate is transformed by ClcB2 to 5-chloromuconolactone, which during turnover by ClcF gives cis-dienelactone as the sole product. cis-Dienelactone was further hydrolyzed by ClcD2 to maleylacetate. ClcF, despite its sequence similarity to muconolactone isomerases, no longer showed muconolactone-isomerizing activity and thus represents an enzyme dedicated to its new function as a 5-chloromuconolactone dehalogenase. Thus, during 3-chlorocatechol degradation by R. opacus 1CP, dechlorination is catalyzed by a muconolactone isomerase-related enzyme rather than by a specialized chloromuconate cycloisomerase.

摘要

先前已证明,4-氯苯酚和2,4-二氯苯酚降解菌株不透明红球菌1CP在长期适应过程中获得了矿化2-氯苯酚的能力。此外,从以2-氯苯酚为生长底物的生物量中提取的均一氯邻苯二酚1,2-双加氧酶对3-氯邻苯二酚表现出相对较高的活性。基于该酶N端和胰蛋白酶肽段的序列,设计了简并PCR引物,用于从菌株1CP的基因组DNA中克隆相应基因。在pROP1上获得了一个包含9个开放阅读框的9.5kb片段。除其他基因外,还鉴定出一个由4个氯邻苯二酚分解代谢基因组成的基因簇。根据序列相似性以及预测的N端与纯化酶的N端的对应性判断,这些开放阅读框分别对应于第二种氯邻苯二酚1,2-双加氧酶(ClcA2)、第二种氯粘康酸环异构酶(ClcB2)、第二种二烯内酯水解酶(ClcD2)和一种与粘康内酯异构酶相关的酶(ClcF)的基因。这个新基因簇的所有酶与已知的氯邻苯二酚酶只有远缘关系,似乎代表了这些活性的新进化谱系。紫外叠加光谱以及高压液相色谱分析证实,2-氯-顺,顺-粘康酸被ClcB2转化为5-氯粘康内酯,在ClcF的周转过程中,5-氯粘康内酯产生顺式二烯内酯作为唯一产物。顺式二烯内酯被ClcD2进一步水解为马来酰乙酸。ClcF尽管其序列与粘康内酯异构酶相似,但不再表现出粘康内酯异构化活性,因此代表一种专门行使其作为5-氯粘康内酯脱卤酶新功能的酶。因此,在不透明红球菌1CP降解3-氯邻苯二酚的过程中,脱氯反应是由一种与粘康内酯异构酶相关的酶催化的,而不是由一种专门的氯粘康酸环异构酶催化的。

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