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Functional analysis of very long-chain fatty acid elongase gene, HpELO2, in the methylotrophic yeast Hansenula polymorpha

机译:甲基营养型酵母多形汉逊酵母中超长链脂肪酸延伸酶基因HpELO2的功能分析

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摘要

We describe the cloning and functional characterization of the fatty acid elongase gene HpELO2, a homologue of the HpELO1 gene required for the production of C24:0 in the yeast Hansenula polymorpha. The open reading frame (ORF) of HpELO2 consists of 1,035 bp, encoding 344 amino acids, sharing about 65% identity with that of Saccharomyces cerevisiae Elo2. Expression of HpELO2 rescued the lethality of the S. cerevisiae elo2 Delta elo3 Delta double disruptant. An accumulation of C18:0 and a significant increase and decrease in the levels of C24:0 and C26:0, respectively, were observed in the Hpelo2 Delta disruptant. These results supported an idea that HpELO2 encodes a fatty acid elongase involved in the elongation of C18:0 to very long-chain fatty acids. The Hpelo1 Delta Hpelo2 Delta double disruption was nonviable, suggesting that HpELO1 and HpELO2 are the only two genes necessary for the biosynthesis in H. polymorpha. Interestingly, transcription of HpELO2 and HpELO1 were found to be transiently up-regulated by exogenous long-chain fatty acids; however, this up-regulation was not observed with HpELO1 and HpELO2 genes driven by the constitutively expressed promoter of the HpACT gene, suggesting that exogenous fatty acids specifically trigger the transcriptional induction of HpELO1 and HpELO2 through their promoter regions.
机译:我们描述了脂肪酸延伸酶基因HpELO2的克隆和功能表征,该基因是酵母多形汉逊酵母中产生C24:0所需的HpELO1基因的同源物。 HpELO2的开放阅读框(ORF)由1,035 bp组成,编码344个氨基酸,与酿酒酵母Elo2具有65%的同一性。 HpELO2的表达挽救了酿酒酵母elo2 Delta elo3 Delta双重破坏物的致死性。在Hpelo2 Delta破坏物中观察到C18:0的积累,以及C24:0和C26:0的水平分别显着增加和减少。这些结果支持了一个想法,即HpELO2编码一种与C18:0延伸至长链脂肪酸有关的脂肪酸延伸酶。 Hpelo1 Delta Hpelo2 Delta双重破坏是不可行的,这表明HpELO1和HpELO2是多形汉逊酵母生物合成所需的仅有的两个基因。有趣的是,HpELO2和HpELO1的转录被外源性长链脂肪酸瞬时上调。但是,在由HpACT基因组成性表达的启动子驱动的HpELO1和HpELO2基因中未观察到这种上调,这表明外源脂肪酸通过其启动子区域特异性触发HpELO1和HpELO2的转录诱导。

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