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来自红色海洋藻类丝状羽藻的一种新型异构酶催化含共轭三烯脂肪酸的生物合成。

Biosynthesis of conjugated triene-containing fatty acids by a novel isomerase from the red marine alga Ptilota filicina.

作者信息

Wise M L, Hamberg M, Gerwick W H

机构信息

Department of Biochemistry and Biophysics, Oregon State University, Corvallis 97331.

出版信息

Biochemistry. 1994 Dec 27;33(51):15223-32. doi: 10.1021/bi00255a002.

DOI:10.1021/bi00255a002
PMID:7803384
Abstract

The biosynthesis of conjugated triene-containing fatty acids by the red alga Ptilota filicina is catalyzed by a novel enzyme, polyenoic fatty acid isomerase. The enzyme has been highly purified and is described here for the first time. Matrix-assisted laser-induced desorption mass spectrometry was used to determine that the major protein in the purified enzyme is composed of similar or identical subunits of M(r) 58,119 Da. The native enzyme emerges with an apparent M(r) of 174,000 Da from a gel permeation chromatography column. While this enzyme catalyzes the formation of conjugated trienes from a variety of polyunsaturated fatty acid precursors [arachidonate ((5Z,8Z,11Z,14Z)- eicosatetraenoate) is converted to (5Z,7E,9E,14Z)-eicosatetraenoate; gamma-linolenate ((6Z,9Z,12Z)-octadecatrienoate) is converted to 6Z,8E,-10E-octadecatrienoate], this occurs most rapidly with eicosapentaenoate [(5Z,7E,9E,14Z,17Z)- eicosapentaenoate], which is likely the native substrate. Through a series of experiments utilizing gamma-linolenates stereospecifically labeled with deuterium, we have determined that the enzyme intramolecularly transfers the bis-allylic pro-S hydrogen from the C11 position to the C13 position. Furthermore, the bis-allylic pro-R hydrogen at C8 in gamma-linolenate is lost to the solvent. Using arachidonate as substrate, we demonstrated that the C11 olefinic position becomes protonated by a solvent-derived proton. There appears to be no requirement for molecular oxygen, and the transformation is catalyzed by this single enzyme.

摘要

红藻丝状鸭毛藻合成含共轭三烯脂肪酸的过程由一种新型酶——多烯脂肪酸异构酶催化。该酶已得到高度纯化,在此首次进行描述。采用基质辅助激光解吸质谱法确定纯化酶中的主要蛋白质由分子量为58,119 Da的相似或相同亚基组成。从凝胶渗透色谱柱中洗脱出来的天然酶的表观分子量为174,000 Da。虽然这种酶能催化多种多不饱和脂肪酸前体生成共轭三烯[花生四烯酸((5Z,8Z,11Z,14Z)-二十碳四烯酸)转化为(5Z,7E,9E,14Z)-二十碳四烯酸;γ-亚麻酸((6Z,9Z,12Z)-十八碳三烯酸)转化为6Z,8E,-10E-十八碳三烯酸],但二十碳五烯酸[ (5Z,7E,9E,14Z,17Z)-二十碳五烯酸]的反应最为迅速,它可能是天然底物。通过一系列利用氘立体特异性标记的γ-亚麻酸的实验,我们确定该酶在分子内将C11位的双烯丙基前-S氢转移至C13位。此外,γ-亚麻酸中C8位的双烯丙基前-R氢会释放到溶剂中。以花生四烯酸为底物时,我们证明C11烯键位置会被溶剂衍生的质子质子化。该反应似乎不需要分子氧,且由这一种酶催化完成转化。

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