Engeland K, Kindl H
Department of Biochemistry, Philipps-University, Marburg, Federal Republic of Germany.
Eur J Biochem. 1991 Mar 28;196(3):699-705. doi: 10.1111/j.1432-1033.1991.tb15868.x.
A delta 3, delta 2-enoyl-CoA isomerase was extracted from fat-degrading cotyledons of cucumber seedlings. The enzyme is required for the degradation of cis-unsaturated fatty acids, e.g. linoleic acid being present in the storage tissue of cucumber seedlings in high amounts. The delta 3, delta 2-enoyl-CoA isomerase was exclusively localized within peroxisomes. Its purification included chromatography on a hydrophobic matrix, a cation exchanger, and on hydroxylapatite. 17,000-fold purification yielded a protein of apparent homogeneity. The isomerase is a homodimer with a Mr of 50,000 and an isoelectric point of pH approximately 8.1. Delta 3, delta 2-Enoyl-CoA isomerase reversibly catalyzes the conversion of both cis-3-enoyl-CoA and trans-3-enoyl-CoA into trans-2-enoyl-CoA. The isomerase exhibited optimal activity at pH 9 and was active with 3-enoyl-CoA species having chain lengths of C6-C12, with cis-hexanoyl-CoA being the most effective substrate. The purified enzyme did not show enoyl-CoA hydratase activity.
从黄瓜幼苗脂肪降解子叶中提取了Δ3,Δ2-烯酰辅酶A异构酶。该酶是顺式不饱和脂肪酸降解所必需的,例如黄瓜幼苗储存组织中大量存在的亚油酸。Δ3,Δ2-烯酰辅酶A异构酶仅定位于过氧化物酶体中。其纯化过程包括在疏水基质、阳离子交换剂和羟基磷灰石上进行层析。经过17000倍的纯化得到了一种表观均一的蛋白质。该异构酶是一种同型二聚体,分子量为50000,等电点约为pH 8.1。Δ3,Δ2-烯酰辅酶A异构酶可逆地催化顺式-3-烯酰辅酶A和反式-3-烯酰辅酶A转化为反式-2-烯酰辅酶A。该异构酶在pH 9时表现出最佳活性,对链长为C6-C12的3-烯酰辅酶A具有活性,其中顺式己酰辅酶A是最有效的底物。纯化后的酶未显示烯酰辅酶A水化酶活性。
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