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拟南芥FAD2基因编码对多不饱和脂质合成至关重要的酶。

Arabidopsis FAD2 gene encodes the enzyme that is essential for polyunsaturated lipid synthesis.

作者信息

Okuley J, Lightner J, Feldmann K, Yadav N, Lark E, Browse J

机构信息

Institute of Biological Chemistry, Washington State University, Pullman 99164-6340.

出版信息

Plant Cell. 1994 Jan;6(1):147-58. doi: 10.1105/tpc.6.1.147.

Abstract

The polyunsaturated fatty acids linoleate and alpha-linolenate are important membrane components and are the essential fatty acids of human nutrition. The major enzyme responsible for the synthesis of these compounds is the plant oleate desaturase of the endoplasmic reticulum, and its activity is controlled in Arabidopsis by the fatty acid desaturation 2 (fad2) locus. A fad2 allele was identified in a population of Arabidopsis in which mutations had been created by T-DNA insertions. Genomic DNA flanking the T-DNA was cloned by plasmid rescue and used to isolate cDNA and genomic clones of FAD2. A cDNA containing the entire FAD2 coding sequence was expressed in fad2 mutant plants and shown to complement the mutant fatty acid phenotype. The deduced amino acid sequence from the cDNA showed homology to other plant desaturases, and this confirmed that FAD2 is the structural gene for the desaturase. Gel blot analyses of FAD2 mRNA levels showed that the gene is expressed throughout the plant and suggest that transcript levels are in excess of the amount needed to account for oleate desaturation. Sequence analysis identified histidine-rich motifs that could contribute to an iron binding site in the cytoplasmic domain of the protein. Such a position would facilitate interaction between the desaturase and cytochrome b5, which is the direct source of electrons for the desaturation reaction, but would limit interaction of the active site with the fatty acyl substrate.

摘要

多不饱和脂肪酸亚油酸酯和α-亚麻酸酯是重要的膜成分,也是人类营养中的必需脂肪酸。负责合成这些化合物的主要酶是内质网的植物油酸去饱和酶,其活性在拟南芥中由脂肪酸去饱和2(fad2)基因座控制。在一个通过T-DNA插入产生突变的拟南芥群体中鉴定出一个fad2等位基因。通过质粒拯救克隆了T-DNA侧翼的基因组DNA,并用于分离FAD2的cDNA和基因组克隆。将包含完整FAD2编码序列的cDNA在fad2突变体植物中表达,并显示其能互补突变体脂肪酸表型。从cDNA推导的氨基酸序列与其他植物去饱和酶具有同源性,这证实FAD2是去饱和酶的结构基因。对FAD2 mRNA水平的凝胶印迹分析表明该基因在整个植物中都有表达,并且表明转录水平超过了解释油酸去饱和所需的量。序列分析鉴定出富含组氨酸的基序,这些基序可能有助于蛋白质胞质结构域中的铁结合位点。这样的位置将促进去饱和酶与细胞色素b5之间的相互作用,细胞色素b5是去饱和反应的直接电子来源,但会限制活性位点与脂肪酰底物的相互作用。

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