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Expression and enzymatic activity of recombinant cytochrome P450 17 alpha-hydroxylase in Escherichia coli.

机译:重组细胞色素P450 17α-羟化酶在大肠杆菌中的表达和酶活性。

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摘要

When the cDNA encoding bovine microsomal 17 alpha-hydroxylase cytochrome P450 (P45017 alpha) containing modifications within the first seven codons which favor expression in Escherichia coli is placed in a highly regulated tac promoter expression plasmid, as much as 16 mg of spectrally detectable P45017 alpha per liter of culture can be synthesized and integrated into E. coli membranes. The known enzymatic activities of bovine P45017 alpha can be reconstituted by addition of purified rat liver NADPH-cytochrome P450 reductase to isolated E. coli membrane fractions containing the recombinant P45017 alpha enzyme. Surprisingly, it is found that E. coli contain an electron-transport system that can substitute for the mammalian microsomal NADPH-cytochrome P450 reductase in supporting both the 17 alpha-hydroxylase and 17,20-lyase activities of P45017 alpha. Thus, not only can E. coli express this eukaryotic membrane protein at relatively high levels, but as evidenced by metabolism of steroids added directly to the cells, the enzyme is catalytically active in vivo. These studies establish E. coli as an efficacious heterologous expression system for structure-function analysis of the cytochrome P450 system.
机译:当将编码前七个密码子中含有有利于在大肠杆菌中表达的修饰的编码牛微粒体17α-羟化酶细胞色素P450(P45017 alpha)的cDNA置于高度调控的tac启动子表达质粒中时,可检测到多达16 mg的可光谱检测的P45017 alpha每升培养物可以合成并整合到大肠杆菌膜中。牛P45017α的已知酶活性可以通过将纯化的大鼠肝脏NADPH-细胞色素P450还原酶添加到含有重组P45017α酶的分离的大肠杆菌膜级分中来重建。令人惊讶地发现,大肠杆菌包含一种电子传输系统,该系统可以替代哺乳动物微粒体NADPH-细胞色素P450还原酶,从而支持P45017α的17α-羟化酶和17,20-裂合酶活性。因此,大肠杆菌不仅可以以相对较高的水平表达该真核膜蛋白,而且正如直接添加到细胞中的类固醇的代谢所证明的那样,该酶在体内具有催化活性。这些研究将大肠杆菌确立为用于细胞色素P450系统结构功能分析的有效异源表达系统。

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