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乙酰羟酸异构还原酶在鼠伤寒沙门氏菌泛酸生物合成中的作用。

Role of acetohydroxy acid isomeroreductase in biosynthesis of pantothenic acid in Salmonella typhimurium.

作者信息

Primerano D A, Burns R O

出版信息

J Bacteriol. 1983 Jan;153(1):259-69. doi: 10.1128/jb.153.1.259-269.1983.

Abstract

Structural genes have been identified for all of the enzymes involved in the biosynthesis of pantothenic acid in Salmonella typhimurium and Escherichia coli K-12, with the exception of ketopantoic acid reductase, which catalyzes the conversion of alpha-ketopantoate to pantoate. The acetohydroxy acid isomeroreductase from S. typhimurium efficiently bound alpha-ketopantoate (K(m) = 0.25 mM) and catalyzed its reduction at 1/20 the rate at which alpha-acetolactate was reduced. Since two enzymes could apparently participate in the synthesis of pantoate, a S. typhimurium ilvC8 strain was mutagenized to derive strains completely blocked in the conversion of alpha-ketopantoate to pantoate. Several isolates were obtained that grew in isoleucine-valine medium supplemented with either pantoate or pantothenate, but not in the same medium supplemented with alpha-ketopantoate or beta-alanine. The mutations that conferred pantoate auxotrophy (designated panE) to these isolates appeared to be clustered, but were not linked to panB or panC. All panE strains tested had greatly reduced levels of ketopantoic acid reductase (3 to 12% of the activity present in DU201). The capacity of the isomeroreductase to synthesize pantoate in vivo was assessed by determining the growth requirements of ilvC(+) derivatives of panE ilvC8 strains. These strains required either alpha-ketopantoate, pantoate, or pantothenate when the isomeroreductase was present at low levels; when the synthesis of isomeroreductase was induced, panE ilvC(+) strains grew in unsupplemented medium. These phenotypes indicate that a high level of isomeroreductase is sufficient for the synthesis of pantoate. panE ilvC(+) strains also grew in medium supplemented with lysine and methionine. This phenotype resembles that of some S. typhimurium ilvG mutants (e.g., DU501) which are partially blocked in the biosynthesis of coenzyme A and are limited for succinyl coenzyme A. panE ilvC(+) strains which lack the acetohydroxy acid synthases required only methionine for growth (in the presence of leucine, isoleucine, and valine). This and other evidence suggested that the synthesis of pantoic acid by isomeroreductase was blocked by the alpha-acetohydroxy acids and that pantoic acid synthesis was enhanced in the absence of these intermediates, even when the isomeroreductase was at low levels. panE ilvC(+) strains reverted to pantothenate independence. Several of these revertants were shown to have elevated isomeroreductase levels under noninduced and induced conditions; the suppressing mutation in each revertant was shown to be closely linked to ilvC by P22 transduction. This procedure presents a means for obtaining mutants with altered regulation of isomeroreductase.

摘要

除了催化α-酮泛解酸转化为泛解酸的酮泛解酸还原酶外,鼠伤寒沙门氏菌和大肠杆菌K-12中参与泛酸生物合成的所有酶的结构基因均已被鉴定。鼠伤寒沙门氏菌的乙酰羟酸异构还原酶能有效结合α-酮泛解酸(K(m)=0.25 mM),并以还原α-乙酰乳酸速率的1/20催化其还原。由于两种酶显然都能参与泛解酸的合成,因此对鼠伤寒沙门氏菌ilvC8菌株进行诱变,以获得在α-酮泛解酸转化为泛解酸过程中完全受阻的菌株。获得了几个分离株,它们在补充了泛解酸或泛酸的异亮氨酸-缬氨酸培养基中生长,但在补充了α-酮泛解酸或β-丙氨酸的相同培养基中不生长。赋予这些分离株泛解酸营养缺陷型(命名为panE)的突变似乎聚集在一起,但与panB或panC不连锁。所有测试的panE菌株的酮泛解酸还原酶水平都大幅降低(为DU201中活性的3%至12%)。通过确定panE ilvC8菌株的ilvC(+)衍生物的生长需求,评估了异构还原酶在体内合成泛解酸的能力。当异构还原酶水平较低时,这些菌株需要α-酮泛解酸、泛解酸或泛酸;当异构还原酶的合成被诱导时,panE ilvC(+)菌株在未补充的培养基中生长。这些表型表明高水平的异构还原酶足以合成泛解酸。panE ilvC(+)菌株在补充了赖氨酸和蛋氨酸的培养基中也能生长。这种表型类似于一些鼠伤寒沙门氏菌ilvG突变体(如DU501),它们在辅酶A的生物合成中部分受阻,并且琥珀酰辅酶A有限。缺乏乙酰羟酸合酶的panE ilvC(+)菌株生长仅需要蛋氨酸(在亮氨酸、异亮氨酸和缬氨酸存在的情况下)。这一点及其他证据表明,异构还原酶合成泛解酸的过程被α-乙酰羟酸阻断,并且在没有这些中间产物的情况下,即使异构还原酶水平较低,泛解酸的合成也会增强。panE ilvC(+)菌株回复为不依赖泛酸。其中一些回复突变体在未诱导和诱导条件下异构还原酶水平均升高;通过P22转导表明每个回复突变体中的抑制突变与ilvC紧密连锁。该方法提供了一种获得异构还原酶调控改变的突变体的手段。

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