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首页> 美国卫生研究院文献>Journal of Bacteriology >Identification of an Archaeal 2-Hydroxy Acid Dehydrogenase Catalyzing Reactions Involved in Coenzyme Biosynthesis in Methanoarchaea
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Identification of an Archaeal 2-Hydroxy Acid Dehydrogenase Catalyzing Reactions Involved in Coenzyme Biosynthesis in Methanoarchaea

机译:甲烷古细菌中参与辅酶生物合成的古细菌2-羟基脱氢酶催化反应的鉴定

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Two putative malate dehydrogenase genes, MJ1425 and MJ0490, from Methanococcus jannaschii and one from Methanothermus fervidus were cloned and overexpressed in Escherichia coli, and their gene products were tested for the ability to catalyze pyridine nucleotide-dependent oxidation and reduction reactions of the following α-hydroxy–α-keto acid pairs: (S)-sulfolactic acid and sulfopyruvic acid; (S)-α-hydroxyglutaric acid and α-ketoglutaric acid; (S)-lactic acid and pyruvic acid; and 1-hydroxy-1,3,4,6-hexanetetracarboxylic acid and 1-oxo-1,3,4,6-hexanetetracarboxylic acid. Each of these reactions is involved in the formation of coenzyme M, methanopterin, coenzyme F420, and methanofuran, respectively. Both the MJ1425-encoded enzyme and the MJ0490-encoded enzyme were found to function to different degrees as malate dehydrogenases, reducing oxalacetate to (S)-malate using either NADH or NADPH as a reductant. Both enzymes were found to use either NADH or NADPH to reduce sulfopyruvate to (S)-sulfolactate, but the Vmax/Km value for the reduction of sulfopyruvate by NADH using the MJ1425-encoded enzyme was 20 times greater than any other combination of enzymes and pyridine nucleotides. Both the M. fervidus and the MJ1425-encoded enzyme catalyzed the NAD+-dependent oxidation of (S)-sulfolactate to sulfopyruvate. The MJ1425-encoded enzyme also catalyzed the NADH-dependent reduction of α-ketoglutaric acid to (S)-hydroxyglutaric acid, a component of methanopterin. Neither of the enzymes reduced pyruvate to (S)-lactate, a component of coenzyme F420. Only the MJ1425-encoded enzyme was found to reduce 1-oxo-1,3,4,6-hexanetetracarboxylic acid, and this reduction occurred only to a small extent and produced an isomer of 1-hydroxy-1,3,4,6-hexanetetracarboxylic acid that is not involved in the biosynthesis of methanofuran c. We conclude that the MJ1425-encoded enzyme is likely to be involved in the biosynthesis of both coenzyme M and methanopterin.
机译:在詹氏甲烷球菌中克隆了两个假定的苹果酸脱氢酶基因MJ1425和MJ0490,在费氏大肠杆菌中克隆了一个苹果酸脱氢酶基因,并在大肠杆菌中过表达,并测试了它们的基因产物催化下列α-核苷酸催化吡啶核苷酸依赖性氧化和还原反应的能力。羟基-α-酮酸对:(S)-磺基乳酸和磺基丙酮酸; (S)-α-羟基戊二酸和α-酮戊二酸; (S)-乳酸和丙酮酸;和1-羟基-1,3,4,6-己四羧酸和1-氧代-1,3,4,6-己四羧酸。这些反应中的每一个都分别参与辅酶M,甲烷蝶呤,辅酶F420和甲氧呋喃的形成。发现MJ1425编码的酶和MJ0490编码的酶都作为苹果酸脱氢酶发挥不同程度的作用,使用NADH或NADPH作为还原剂将草酰乙酸还原为(S)-苹果酸。发现这两种酶都使用NADH或NADPH来将硫代丙酮酸还原为(S)-巯基乳酸,但使用MJ1425编码的酶通过NADH还原硫代丙酮酸的Vmax / Km值比任何其他酶组合高20倍。吡啶核苷酸。狂犬分枝杆菌和MJ1425编码的酶都催化(S)-巯基乳酸NAD + 依赖的氧化为硫代丙酮酸。 MJ1425编码的酶还催化依赖NADH的α-酮戊二酸还原为(S)-羟基戊二酸(一种甲烷蝶呤)。两种酶都没有将丙酮酸还原为(S)-乳酸,这是辅酶F420的组成部分。仅发现MJ1425-编码的酶还原1-oxo-1,3,4,6-己四羧酸,并且这种还原仅在很小的程度上发生,并产生1-羟基-1,3,4,6的异构体。不参与甲烷呋喃c的生物合成的-己烷四甲酸。我们得出的结论是,MJ1425编码的酶可能与辅酶M和甲烷蝶呤的生物合成有关。

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