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甘氨酸裂解系统成熟牛H蛋白在大肠杆菌中的表达及脱辅基形式的体外脂酰化作用。

Expression of mature bovine H-protein of the glycine cleavage system in Escherichia coli and in vitro lipoylation of the apoform.

作者信息

Fujiwara K, Okamura-Ikeda K, Motokawa Y

机构信息

Institute for Enzyme Research, University of Tokushima, Japan.

出版信息

J Biol Chem. 1992 Oct 5;267(28):20011-6.

PMID:1400316
Abstract

H-protein, a component of the glycine cleavage system with lipoic acid as a prosthetic group, was expressed in Escherichia coli using a T7 RNA polymerase plasmid expression system. After induction with 25 microM isopropyl-beta-D-thiogalactopyranoside, bacteria harboring the recombinant plasmid expressed mature bovine H-protein as a soluble form at a level of about 10% of the total bacterial protein. Little of the H-protein was lipoylated in E. coli cultured without added lipoate, but when the cells were cultured in medium supplemented with 30 microM lipoate, about 10% of the recombinant protein expressed was the correctly lipoylated active form, 10% was an inactive aberrantly modified form, presumably with an octanoyl group, and the remaining 80% was the unlipoylated apoform. Each of the three forms was purified to homogeneity and shown to have the same NH2-terminal amino acid sequence as that of native bovine H-protein. The specific activity of the lipoylated form of H-protein expressed was consistent with that of H-protein purified from bovine liver. The purified recombinant apo-H-protein was lipoylated and consequently activated in vitro with lipoyl-AMP as a lipoyl donor by lipoyltransferase purified 150-fold from bovine liver mitochondria. The lipoylation was dependent on lipoyl-AMP, apo-H-protein, and lipoyltransferase. The partially purified lipoyltransferase had no lipoate-activating activity. These results provide the first evidence that in mammals two consecutive reactions are required for the attachment of lipoic acid to the acceptor protein: the activation of lipoic acid to lipoyl-AMP catalyzed by lipoate-activating enzyme and the transfer of the lipoyl group to an N epsilon-amino group of a lysine residue to apoprotein by lipoyl-AMP:N epsilon-lysine lipoyltransferase.

摘要

H蛋白是甘氨酸裂解系统的一个组成部分,以硫辛酸为辅基,利用T7 RNA聚合酶质粒表达系统在大肠杆菌中表达。用25微摩尔异丙基-β-D-硫代半乳糖苷诱导后,携带重组质粒的细菌以可溶性形式表达成熟的牛H蛋白,其水平约占细菌总蛋白的10%。在不添加硫辛酸的培养基中培养的大肠杆菌中,很少有H蛋白被硫辛酰化,但当细胞在添加了30微摩尔硫辛酸的培养基中培养时,表达的重组蛋白中约10%是正确硫辛酰化的活性形式,10%是无活性的异常修饰形式,可能带有辛酰基,其余80%是未硫辛酰化的脱辅基形式。这三种形式均被纯化至同质,并显示其NH2末端氨基酸序列与天然牛H蛋白相同。表达的硫辛酰化形式的H蛋白的比活性与从牛肝中纯化的H蛋白一致。纯化的重组脱辅基H蛋白在体外被硫辛酰化,并通过从牛肝线粒体中纯化150倍的硫辛酰转移酶,以硫辛酰-AMP作为硫辛酰供体而被激活。硫辛酰化依赖于硫辛酰-AMP、脱辅基H蛋白和硫辛酰转移酶。部分纯化的硫辛酰转移酶没有硫辛酸激活活性。这些结果首次证明,在哺乳动物中,硫辛酸与受体蛋白的连接需要两个连续反应:硫辛酸激活酶催化硫辛酸激活为硫辛酰-AMP,以及硫辛酰-AMP:Nε-赖氨酸硫辛酰转移酶将硫辛酰基转移至脱辅基蛋白赖氨酸残基的Nε-氨基上。

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