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对硫辛酸的硒类似物具有抗性的大肠杆菌K-12突变体可鉴定硫辛酸代谢中的未知基因。

Mutants of Escherichia coli K-12 that are resistant to a selenium analog of lipoic acid identify unknown genes in lipoate metabolism.

作者信息

Reed K E, Morris T W, Cronan J E

机构信息

Department of Microbiology, University of Illinois at Urbana-Champaign 61801.

出版信息

Proc Natl Acad Sci U S A. 1994 Apr 26;91(9):3720-4. doi: 10.1073/pnas.91.9.3720.

Abstract

Lipoic acid is a disulfide-containing cofactor required for the reactions catalyzed by alpha-ketoacid dehydrogenase enzyme complexes. We report the chemical synthesis and biological properties of lipoic acid analogs in which one or both sulfur atoms were replaced by selenium. Replacement of either the C-6 or the C-8 sulfur atom with selenium results in lipoic acid derivatives with apparently unaltered biological properties. However, simultaneous replacement of both sulfur atoms gave an analog (selenolipoic acid) that inhibited growth of wild-type Escherichia coli when present in minimal glucose medium at 50 ng/ml. This growth inhibition was reversed by the addition of either excess lipoic acid or acetate plus succinate. Labeling experiments with [75Se]selenolipoic acid showed that this compound was efficiently incorporated into the alpha-ketoacid dehydrogenase complexes of growing cells. Spontaneously arising selenolipoic acid-resistant (slr) mutants were isolated. Two of these isolates resistant to high levels of selenolipoic acid were studied in detail. The slr-1 mutation, which was mapped to min 99.6 of the E. coli chromosome, increased the lipoate requirement of lipA strains by 4-fold and appeared to define a gene encoding a lipoate-protein ligase. The slr-7 mutation, which was mapped to min 15.25 of the chromosome, completely suppressed the lipoate requirement of lipA strains and defined a gene of unknown function in the synthesis of lipoic acid.

摘要

硫辛酸是α-酮酸脱氢酶复合体催化反应所需的一种含二硫键的辅因子。我们报道了硫辛酸类似物的化学合成及其生物学特性,其中一个或两个硫原子被硒取代。用硒取代C-6或C-8硫原子会产生生物学特性明显未改变的硫辛酸衍生物。然而,同时取代两个硫原子得到一种类似物(硒代硫辛酸),当在最低葡萄糖培养基中以50 ng/ml存在时,它会抑制野生型大肠杆菌的生长。添加过量硫辛酸或乙酸盐加琥珀酸盐可逆转这种生长抑制。用[75Se]硒代硫辛酸进行的标记实验表明,该化合物能有效地掺入生长细胞的α-酮酸脱氢酶复合体中。分离出了自发产生的抗硒代硫辛酸(slr)突变体。对其中两个对高浓度硒代硫辛酸有抗性的分离株进行了详细研究。slr-1突变定位在大肠杆菌染色体的99.6分钟处,使lipA菌株对硫辛酸的需求增加了4倍,似乎定义了一个编码硫辛酸-蛋白连接酶的基因。slr-7突变定位在染色体的15.25分钟处,完全抑制了lipA菌株对硫辛酸的需求,并在硫辛酸合成中定义了一个功能未知的基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/95ee/43653/9ef00dc042d5/pnas01131-0254-a.jpg

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