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酿酒酵母LPP1基因的分离与鉴定,该基因编码一种不依赖镁离子的磷脂酸磷酸酶。

Isolation and characterization of the Saccharomyces cerevisiae LPP1 gene encoding a Mg2+-independent phosphatidate phosphatase.

作者信息

Toke D A, Bennett W L, Oshiro J, Wu W I, Voelker D R, Carman G M

机构信息

Department of Food Science, Cook College, New Jersey Agricultural Experiment Station, Rutgers University, New Brunswick, New Jersey 08903, USA.

出版信息

J Biol Chem. 1998 Jun 5;273(23):14331-8. doi: 10.1074/jbc.273.23.14331.

Abstract

The DPP1-encoded diacylglycerol pyrophosphate (DGPP) phosphatase enzyme accounts for half of the Mg2+-independent phosphatidate (PA) phosphatase activity in Saccharomyces cerevisiae. The LPP1 (lipid phosphate phosphatase) gene encodes a protein that contains a novel phosphatase sequence motif found in DGPP phosphatase and in the mouse Mg2+-independent PA phosphatase. A genomic copy of the S. cerevisiae LPP1 gene was isolated and was used to construct lpp1Delta and lpp1Delta dpp1Delta mutants. A multicopy plasmid containing the LPP1 gene directed a 12.9-fold overexpression of Mg2+-independent PA phosphatase activity in the S. cerevisiae lpp1Delta dpp1Delta double mutant. The heterologous expression of the S. cerevisiae LPP1 gene in Sf-9 insect cells resulted in a 715-fold overexpression of Mg2+-independent PA phosphatase activity relative to control insect cells. The Mg2+-independent PA phosphatase activity encoded by the LPP1 gene was associated with the membrane fraction of the cell. The LPP1 gene product also exhibited lyso-PA phosphatase and DGPP phosphatase activities. The order of substrate preference was PA > lyso-PA > DGPP. Like the dpp1Delta mutant, the lpp1Delta mutant and the lpp1Delta dpp1Delta double mutant were viable and did not exhibit obvious growth defects. Biochemical analyses of lpp1Delta, dpp1Delta, and lpp1Delta dpp1Delta mutants showed that the LPP1 and DPP1 gene products encoded nearly all of the Mg2+-independent PA phosphatase and lyso-PA phosphatase activities and all of the DGPP phosphatase activity in S. cerevisiae. Moreover, the analyses of the mutants showed that the LPP1 and DPP1 gene products played a role in the regulation of phospholipid metabolism and the cellular levels of phosphatidylinositol and PA.

摘要

由DPP1编码的二酰基甘油焦磷酸(DGPP)磷酸酶占酿酒酵母中不依赖Mg2+的磷脂酸(PA)磷酸酶活性的一半。LPP1(脂质磷酸磷酸酶)基因编码一种蛋白质,该蛋白质含有在DGPP磷酸酶和小鼠不依赖Mg2+的PA磷酸酶中发现的新型磷酸酶序列基序。分离出酿酒酵母LPP1基因的基因组拷贝,并用于构建lpp1Δ和lpp1Δ dpp1Δ突变体。含有LPP1基因的多拷贝质粒在酿酒酵母lpp1Δ dpp1Δ双突变体中使不依赖Mg2+的PA磷酸酶活性过表达了12.9倍。酿酒酵母LPP1基因在Sf-9昆虫细胞中的异源表达导致相对于对照昆虫细胞,不依赖Mg2+的PA磷酸酶活性过表达了715倍。由LPP1基因编码的不依赖Mg2+的PA磷酸酶活性与细胞的膜部分相关。LPP1基因产物还表现出溶血磷脂酸磷酸酶和DGPP磷酸酶活性。底物偏好顺序为PA>溶血磷脂酸>DGPP。与dpp1Δ突变体一样,lpp1Δ突变体和lpp1Δ dpp1Δ双突变体是有活力的,并且没有表现出明显的生长缺陷。对lpp1Δ、dpp1Δ和lpp1Δ dpp1Δ突变体的生化分析表明,LPP1和DPP1基因产物编码了酿酒酵母中几乎所有不依赖Mg2+的PA磷酸酶和溶血磷脂酸磷酸酶活性以及所有的DGPP磷酸酶活性。此外,对突变体的分析表明,LPP1和DPP1基因产物在磷脂代谢以及磷脂酰肌醇和PA的细胞水平调节中发挥作用。

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