首页> 外文期刊>Journal of Agricultural and Food Chemistry >Cloning and Characterization of a Catechol-Degrading Gene Cluster from 3,4-dichloroaniline Degrading Bacterium Pseudomonas sp. KB35B
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Cloning and Characterization of a Catechol-Degrading Gene Cluster from 3,4-dichloroaniline Degrading Bacterium Pseudomonas sp. KB35B

机译:从3,4-二氯苯胺降解细菌假单胞菌sp。的降解邻苯二酚的基因簇的克隆和鉴定。 KB35B

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摘要

We recently isolated a bacterium, Pseudomonas sp. KB35B, capable of growth on 3,4-dichloroaniline (DCA) as a sole carbon source. The isolated strain showed a high level of catechol 2,3-dioxygenase (CD-2,3) activity in the presence of 3,4-DCA. In an attempt to elucidate the relationship between biodegradation of 3,4-DCA and CD-2,3 activity, the genes encoding enzymes for the catabolic pathway of catechol were cloned and sequenced from the chromosomal DNA. The sequence analysis of the 10752 bp DNA fragment revealed 12 open reading frames in the order of nahRGTHINLOMKJX. Among the 12 genes, nahHINLOMK genes encode enzymes for the metabolism of catechol to TCA cycle intermediates. The nahR gene is the LysR type transcriptional regulator, and the nahH gene encodes CD-2,3 for mefa-cleavages of catechol. 2-Hydroxymuconic semialdehyde hydrolase, 2-oxypent-4-dienoate hydratase, and 4-hydroxy-2-oxovalerate aldolase encoded by nahLMN genes are responsible for the three steps after mefa-cleavages of catechol. The current results suggested that Pseudomonas sp. KB35B degrades 3,4-DCA via the mefa-cleavage pathway of catechol.
机译:我们最近分离出了一种细菌,假单胞菌。 KB35B,能够在3,4-二氯苯胺(DCA)上作为唯一碳源生长。在3,4-DCA存在下,分离出的菌株显示出高水平的儿茶酚2,3-二加氧酶(CD-2,3)活性。为了阐明3,4-DCA的生物降解与CD-2,3活性之间的关系,从染色体DNA克隆了编码儿茶酚分解途径的酶的基因并进行了测序。 10752 bp DNA片段的序列分析揭示了以nahRGTHINLOMKJX的顺序排列的12个开放阅读框。在这12个基因中,nahHINLOMK基因编码用于将儿茶酚代谢为TCA循环中间体的酶。 nahR基因是LysR型转录调节子,而nahH基因编码CD-2,3用于儿茶酚的mefa裂解。 nahLMN基因编码的2-羟基粘康半醛水解酶,2-氧基戊-4-二烯酸酯水合酶和4-羟基-2-氧戊醛醛缩醛酶负责儿茶酚的甲乙酰胺裂解后的三个步骤。目前的结果表明假单胞菌属。 KB35B通过儿茶酚的mefa裂解途径降解3,4-DCA。

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