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Characterization of the catabolic pathway for a phenylcoumaran-type lignin-derived biaryl in Sphingobium sp strain SYK-6

机译:鞘氨醇单胞菌菌株SYK-6中苯香豆素型木质素衍生联芳的分解代谢途径的表征

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Sphingobium sp. strain SYK-6 is capable of degrading various lignin-derived biaryls. We determined the catabolic pathway of a phenylcoumaran-type compound, dehydrodiconiferyl alcohol (DCA) in SYK-6, and identified some of the DCA catabolism genes. In SYK-6 cells, the alcohol group of DCA was oxidized to the carboxyl group, first at the B-ring side chain and then at the A-ring side chain. The resultant metabolite was degraded to 5-formylferulate and vanillin through the decarboxylation and the C alpha-C beta cleavage of the A-ring side chain. Based on the DCA catabolic pathway, alcohol dehydrogenase (ADH) and aldehyde dehydrogenase (ALDH) genes are thought to be involved in the conversion of DCA into an aldehyde intermediate (DCA-L) and the conversion of DCA-L into a carboxylic acid intermediate (DCA-C), respectively. SLG_05620 and SLG_24930, which belong to quinohemoprotein ADH and aryl ADH, respectively, were isolated as the genes responsible for the oxidation of DCA. In addition to these genes, multiple genes similar to SLG_05620 and SLG_24930 were found to confer DCA oxidation activities on Escherichia coli cells. In order to identify the DCA-L dehydrogenase genes, the DCA-L oxidation activities of the SYK-6 gene products of putative twenty-one ALDH genes were examined. Significant activities were observed in the four ALDH gene products, including the SLG_27910 product, which showed the highest activity. The disruption of SLG_27910 caused a decreased conversion of DCA-L, suggesting that SLG_27910 plays an important role in the DCA-L oxidation. In conclusion, no specific gene seems to be solely responsible for the conversion of DCA and DCA-L, however, the multiple genes encoding quinohemoprotein ADH and aryl ADH genes, and four ALDH genes are probably involved in the conversion processes
机译:鞘氨醇单胞菌SYK-6菌株能够降解各种木质素衍生的联芳基。我们确定了SYK-6中的苯并香豆素类化合物,去氢二烯基壬二醇(DCA)的分解代谢途径,并鉴定了一些DCA分解代谢基因。在SYK-6细胞中,DCA的醇基首先在B环侧链然后在A环侧链被氧化为羧基。所得代谢物通过A环侧链的脱羧作用和C alpha-C beta裂解而降解为5-甲酰基阿魏酸酯和香草醛。基于DCA分解代谢途径,醇脱氢酶(ADH)和醛脱氢酶(ALDH)基因被认为与DCA转化为醛中间体(DCA-L)和DCA-L转化为羧酸中间体有关(DCA-C)。分离出分别属于喹血红蛋白ADH和芳基ADH的SLG_05620和SLG_24930作为负责DCA氧化的基因。除了这些基因之外,还发现了多个类似于SLG_05620和SLG_24930的基因,这些基因赋予大肠杆菌细胞DCA氧化活性。为了鉴定DCA-L脱氢酶基因,检查了推定的21个ALDH基因的SYK-6基因产物的DCA-L氧化活性。在四个ALDH基因产物(包括SLG_27910产物)中观察到了显着的活性,这些产物显示出最高的活性。 SLG_27910的破坏导致DCA-L的转化降低,这表明SLG_27910在DCA-L的氧化中起着重要的作用。总之,似乎没有特定基因单独负责DCA和DCA-L的转化,但是,编码喹诺蛋白ADH和芳基ADH基因的多个基因以及四个ALDH基因可能参与了转化过程

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