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首页> 外文期刊>Antonie van Leeuwenhoek: Journal of Microbiology and serology >Expression control of nitrile hydratase and amidase genes in Rhodococcus erythropolis and substrate specificities of the enzymes
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Expression control of nitrile hydratase and amidase genes in Rhodococcus erythropolis and substrate specificities of the enzymes

机译:红球红球菌腈水合酶和酰胺酶基因的表达控制及该酶的底物特异性

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摘要

Bacterial amidases and nitrile hydratases can be used for the synthesis of various intermediates and products in the chemical and pharmaceutical industries and for the bioremediation of toxic pollutants. The aim of this study was to analyze the expression of the amidase and nitrile hydratase genes of Rhodococcus erythropolis and test the stereospecific nitrile hydratase and amidase activities on chiral cyanohydrins. The nucleotide sequences of the gene clusters containing the oxd (aldoxime dehydratase), ami (amidase), nha1, nha2 (subunits of the nitrile hydratase), nhr1, nhr2, nhr3 and nhr4 (putative regulatory proteins) genes of two R. erythropolis strains, A4 and CCM2595, were determined. All genes of both of the clusters are transcribed in the same direction. RT-PCR analysis, primer extension and promoter fusions with the gfp reporter gene showed that the ami, nha1 and nha2 genes of R. erythropolis A4 form an operon transcribed from the Pami promoter and an internal Pnha promoter. The activity of Pami was found to be weakly induced when the cells grew in the presence of acetonitrile, whereas the Pnha promoter was moderately induced by both the acetonitrile or acetamide used instead of the inorganic nitrogen source. However, R. erythropolis A4 cells showed no increase in amidase and nitrile hydratase activities in the presence of acetamide or acetonitrile in the medium. R. erythropolis A4 nitrile hydratase and amidase were found to be effective at hydrolysing cyanohydrins and 2-hydroxyamides, respectively.
机译:细菌酰胺酶和腈水合酶可用于化学和制药工业中各种中间体和产品的合成,以及有毒污染物的生物修复。这项研究的目的是分析红红球菌的酰胺酶和腈水合酶基因的表达,并测试立体特异性腈水合酶和酰胺酶对手性氰醇的活性。基因簇的核苷酸序列,包含两个R. erythropolis菌株的oxd(醛肟脱水酶),ami(酰胺酶),nha1,nha2(腈水合酶的亚基),nhr1,nhr2,nhr3和nhr4(假定的调节蛋白)基因。确定了A4和CCM2595。两个簇的所有基因都沿相同方向转录。 RT-PCR分析,引物延伸和启动子与gfp报告基因的融合表明,红球菌A4的ami,nha1和nha2基因形成从Pami启动子和内部Pnha启动子转录的操纵子。当细胞在乙腈存在下生长时,发现Pami的活性被弱诱导,而Pnha启动子被乙腈或乙酰胺(而不是无机氮源)适度诱导。但是,在培养基中存在乙酰胺或乙腈的情况下,R。erythropolis A4细胞未显示酰胺酶和腈水合酶活性的增加。发现R. erythropolis A4腈水合酶和酰胺酶分别有效水解氰醇和2-羟酰胺。

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