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首页> 外文期刊>Fungal Genetics and Biology >Functional roles and substrate specificities of twelve cytochromes P450 belonging to CYP52 family in n-alkane assimilating yeast Yarrowia lipolytica
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Functional roles and substrate specificities of twelve cytochromes P450 belonging to CYP52 family in n-alkane assimilating yeast Yarrowia lipolytica

机译:十二种属于CYP52家族的细胞色素P450在正构烷烃消化酵母解脂耶氏酵母中的功能和底物特异性

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Yarrowia lipolytica possesses twelve ALK genes, which encode cytochromes P450 in the CYP52 family. In this study, using a Y. lipolytica strain from which all twelve ALK genes had been deleted, strains individually expressing each of the ALK genes were constructed and their roles and substrate specificities were determined by observing their growth on n-alkanes and analyzing fatty acid metabolism. The results suggested that the twelve Alk proteins can be categorized into four groups based on their substrate specificity: Alk1p, Alk2p, Alk9p, and Alk10p, which have significant activities to hydroxylate n-alkanes; Alk4p, Alk5p, and Alk7p, which have significant activities to hydroxylate the co-terminal end of dodecanoic acid; Alk3p and Alk6p, which have significant activities to hydroxylate both n-alkanes and dodecanoic acid; and Alk8p, Alk11p, and Alk12p, which showed faint or no activities to oxidize these substrates. The involvement of Alk proteins in the oxidation of fatty alcohols and fatty aldehydes was also analyzed by measuring viability of the mutant deleted for twelve ALK genes in medium containing dodecanol and by observing growth on dodecanal of a mutant strain, in which twelve ALK genes were deleted along with four fatty aldehyde dehydrogenase genes. It was suggested that ALK gene(s) is/are involved in the detoxification of dodecanol and the assimilation of dodecanal. These results imply that genes encoding CYP52-family P450s have undergone multiplication and diversification in Y. lipolytica for assimilation of various hydrophobic compounds. (C) 2016 Elsevier Inc. All rights reserved.
机译:解脂耶氏酵母具有十二个ALK基因,其编码CYP52家族中的细胞色素P450。在这项研究中,使用解脂耶氏酵母菌株,其中删除了所有12个ALK基因,构建了分别表达每个ALK基因的菌株,并通过观察它们在正构烷烃上的生长并分析脂肪酸来确定其作用和底物特异性。代谢。结果表明,根据其底物特异性,可将十二种Alk蛋白分为四类:Alk1p,Alk2p,Alk9p和Alk10p,它们对羟基化正构烷烃具有显着的活性。 Alk4p,Alk5p和Alk7p,它们具有使十二烷酸的共末端羟基化的显着活性; Alk3p和Alk6p具有显着的使正构烷烃和十二烷酸羟基化的活性;和Alk8p,Alk11p和Alk12p,它们显示出微弱的氧化或没有氧化这些底物的活性。还通过测量缺失十二烷基醇的培养基中十二个ALK基因缺失的突变体的存活力,并观察突变体菌株十二烷的生长,分析了Alk蛋白在脂肪醇和脂肪醛氧化中的参与。以及四个脂肪醛脱氢酶基因。提示ALK基因参与十二烷醇的解毒和十二烷的同化。这些结果暗示编码CYP52家族P450的基因已经在解脂耶氏酵母中经历了繁殖和多样化,以同化各种疏水性化合物。 (C)2016 Elsevier Inc.保留所有权利。

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