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乳酰谷胱甘肽裂解酶是甲基乙二醛解毒过程中的一种关键酶,有助于沙门氏菌在营养丰富的环境中存活。

Lactoylglutathione lyase, a critical enzyme in methylglyoxal detoxification, contributes to survival of Salmonella in the nutrient rich environment.

作者信息

Chakraborty Sangeeta, Gogoi Mayuri, Chakravortty Dipshikha

机构信息

a Department of Microbiology and Cell Biology ; Indian Institute of Science ; Bangalore , India.

出版信息

Virulence. 2015;6(1):50-65. doi: 10.4161/21505594.2014.983791.

Abstract

Glyoxalase I which is synonymously known as lactoylglutathione lyase is a critical enzyme in methylglyoxal (MG) detoxification. We assessed the STM3117 encoded lactoylglutathione lyase (Lgl) of Salmonella Typhimurium, which is known to function as a virulence factor, due in part to its ability to detoxify methylglyoxal. We found that STM3117 encoded Lgl isomerises the hemithioacetal adduct of MG and glutathione (GSH) into S-lactoylglutathione. Lgl was observed to be an outer membrane bound protein with maximum expression at the exponential growth phase. The deletion mutant of S. Typhimurium (Δlgl) exhibited a notable growth inhibition coupled with oxidative DNA damage and membrane disruptions, in accordance with the growth arrest phenomenon associated with typical glyoxalase I deletion. However, growth in glucose minimal medium did not result in any inhibition. Endogenous expression of recombinant Lgl in serovar Typhi led to an increased resistance and growth in presence of external MG. Being a metalloprotein, Lgl was found to get activated maximally by Co(2+) ion followed by Ni(2+), while Zn(2+) did not activate the enzyme and this could be attributed to the geometry of the particular protein-metal complex attained in the catalytically active state. Our results offer an insight on the pivotal role of the virulence associated and horizontally acquired STM3117 gene in non-typhoidal serovars with direct correlation of its activity in lending survival advantage to Salmonella spp.

摘要

乙二醛酶I,也被称为乳酰谷胱甘肽裂解酶,是甲基乙二醛(MG)解毒过程中的关键酶。我们评估了鼠伤寒沙门氏菌中由STM3117编码的乳酰谷胱甘肽裂解酶(Lgl),该酶已知作为一种毒力因子发挥作用,部分原因是其具有解毒甲基乙二醛的能力。我们发现,STM3117编码的Lgl可将MG与谷胱甘肽(GSH)的半硫代缩醛加合物异构化为S-乳酰谷胱甘肽。Lgl被观察到是一种外膜结合蛋白,在指数生长期表达量最高。鼠伤寒沙门氏菌的缺失突变体(Δlgl)表现出显著的生长抑制,并伴有氧化性DNA损伤和膜破坏,这与典型乙二醛酶I缺失相关的生长停滞现象一致。然而,在葡萄糖基本培养基中生长并未导致任何抑制。重组Lgl在伤寒血清型中的内源性表达导致在存在外部MG的情况下抗性增加和生长。作为一种金属蛋白,发现Lgl在Co(2+)离子作用下最大程度地被激活,其次是Ni(2+),而Zn(2+)不能激活该酶,这可能归因于在催化活性状态下所形成的特定蛋白质-金属复合物的几何结构。我们的结果为毒力相关且水平获得的STM3117基因在非伤寒血清型中的关键作用提供了见解,其活性与沙门氏菌属获得生存优势直接相关。

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