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酿酒酵母中影响脂肪酸去饱和作用的OLE1基因的分离与特性分析

Isolation and characterization of OLE1, a gene affecting fatty acid desaturation from Saccharomyces cerevisiae.

作者信息

Stukey J E, McDonough V M, Martin C E

机构信息

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

出版信息

J Biol Chem. 1989 Oct 5;264(28):16537-44.

PMID:2674136
Abstract

The unsaturated fatty acid (ufa) requiring ole1 mutant of Saccharomyces cerevisiae appears to produce a defective delta-9 fatty acid desaturase. This enzyme catalyzes double bond formation between carbons 9 and 10 of palmitoyl and stearoyl coenzyme A. A DNA fragment isolated by complementation of an ole1 strain repairs the ufa requirement in mutant cells. Genetic analysis of the cloned DNA fragment indicates that it is allelic to the OLE1 gene. Disruption of a single copy of the wild type gene in a diploid strain produces both wild type and nonreverting ufa-requiring haploid progeny upon sporulation. Membrane lipids of the disrupted haploid strains contain only ufas supplied in the growth medium. The recovery of activity in both wild type and disrupted segregants was examined after removal of ufas from the growth medium. Following ufa deprivation disruptant cells grew normally for about three generations and then at a slower rate for at least 0.6 generations. During that time cellular ufas dropped from 63 to 7.3 mol % of the total fatty acids. No production of the 16:1 and 18:1 products of the desaturase was observed in disruptant cells, whereas desaturation in wild type control cells was evident 2 h after deprivation. These results indicate that 1) the OLE1 gene is essential for production of monounsaturated fatty acids and is probably the structural gene for the delta-9 desaturase enzyme. 2) A large part of membrane ufas present under normal culture conditions are not essential for growth and cell division.

摘要

酿酒酵母中需要不饱和脂肪酸(ufa)的ole1突变体似乎产生了有缺陷的δ-9脂肪酸去饱和酶。该酶催化棕榈酰辅酶A和硬脂酰辅酶A的碳9和碳10之间形成双键。通过ole1菌株互补分离得到的一个DNA片段修复了突变细胞对ufa的需求。对克隆的DNA片段进行遗传分析表明,它与OLE1基因等位。在二倍体菌株中破坏单个野生型基因的拷贝,在孢子形成后会产生野生型和不能回复的需要ufa的单倍体后代。被破坏的单倍体菌株的膜脂仅含有生长培养基中提供的ufa。在从生长培养基中去除ufa后,检测了野生型和被破坏的分离株中活性的恢复情况。在ufa缺乏后,被破坏的细胞正常生长约三代,然后以较慢的速度生长至少0.6代。在此期间,细胞ufa从总脂肪酸的63%降至7.3%。在被破坏的细胞中未观察到去饱和酶的16:1和18:1产物的产生,而在野生型对照细胞中,在缺乏ufa 2小时后去饱和现象明显。这些结果表明:1)OLE1基因对于单不饱和脂肪酸的产生至关重要,可能是δ-9去饱和酶的结构基因。2)在正常培养条件下存在的大部分膜ufa对于生长和细胞分裂并非必不可少。

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