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ELO2和ELO3是酿酒酵母ELO1基因的同源物,在脂肪酸延长过程中发挥作用,是鞘脂形成所必需的。

ELO2 and ELO3, homologues of the Saccharomyces cerevisiae ELO1 gene, function in fatty acid elongation and are required for sphingolipid formation.

作者信息

Oh C S, Toke D A, Mandala S, Martin C E

机构信息

Bureau of Biological Research, Rutgers University, Nelson Laboratories, Piscataway, New Jersey 08855-1059, USA.

出版信息

J Biol Chem. 1997 Jul 11;272(28):17376-84. doi: 10.1074/jbc.272.28.17376.

DOI:10.1074/jbc.272.28.17376
PMID:9211877
Abstract

ELO2 and ELO3 were identified from the Saccharomyces cerevisiae genome data base as homologues of ELO1, a gene involved in the elongation of the fatty acid 14:0 to 16:0. Mutations in these genes have previously been shown to produce pleiotropic effects involving a number of membrane functions. The simultaneous disruption of ELO2 and ELO3 has also been shown to produce synthetic lethality, indicating that they have related and/or overlapping functions. Gas chromatography and gas chromatography/mass spectroscopy analyses reveal that null mutations of ELO2 and ELO3 produce defects in the formation of very long chain fatty acids. Analysis of the null mutants indicates that these genes encode components of the membrane-bound fatty acid elongation systems that produce the 26-carbon very long chain fatty acids that are precursors for ceramide and sphingolipids. Elo2p appears to be involved in the elongation of fatty acids up to 24 carbons. It appears to have the highest affinity for substrates with chain lengths less than 22 carbons. Elo3p apparently has a broader substrate specificity and is essential for the conversion of 24-carbon acids to 26-carbon species. Disruption of either gene reduces cellular sphingolipid levels and results in the accumulation of the long chain base, phytosphingosine. Null mutations in ELO3 result in accumulation of labeled precursors into inositol phosphoceramide, with little labeling in the more complex mannosylated sphingolipids, whereas disruption of ELO2 results in reduced levels of all sphingolipids.

摘要

ELO2和ELO3是从酿酒酵母基因组数据库中鉴定出来的,它们是ELO1的同源物,ELO1是一个参与将脂肪酸14:0延长至16:0的基因。此前已表明,这些基因的突变会产生涉及多种膜功能的多效性作用。同时破坏ELO2和ELO3也已显示会产生合成致死性,这表明它们具有相关和/或重叠的功能。气相色谱和气相色谱/质谱分析表明,ELO2和ELO3的无效突变会在极长链脂肪酸的形成过程中产生缺陷。对无效突变体的分析表明,这些基因编码膜结合脂肪酸延长系统的组分,该系统产生26碳的极长链脂肪酸,这些脂肪酸是神经酰胺和鞘脂的前体。Elo2p似乎参与了长达24个碳的脂肪酸的延长。它似乎对链长小于22个碳的底物具有最高亲和力。Elo3p显然具有更广泛的底物特异性,并且对于将24碳的酸转化为26碳的酸是必不可少的。破坏任何一个基因都会降低细胞鞘脂水平,并导致长链碱植物鞘氨醇的积累。ELO3的无效突变会导致标记前体积累到肌醇磷酸神经酰胺中,而在更复杂的甘露糖基化鞘脂中标记很少,而ELO2的破坏会导致所有鞘脂水平降低。

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