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内源性金属卟啉插入人膜细胞色素 P450 酶。

Endogenous insertion of non-native metalloporphyrins into human membrane cytochrome P450 enzymes.

机构信息

From the Departments of Medicinal Chemistry and.

From the Departments of Medicinal Chemistry and

出版信息

J Biol Chem. 2018 Oct 26;293(43):16623-16634. doi: 10.1074/jbc.RA118.005417. Epub 2018 Sep 14.

Abstract

Human cytochrome P450 enzymes are membrane-bound heme-containing monooxygenases. As is the case for many heme-containing enzymes, substitution of the metal in the center of the heme can be useful for mechanistic and structural studies of P450 enzymes. For many heme proteins, the iron protoporphyrin prosthetic group can be extracted and replaced with protoporphyrin containing another metal, but human membrane P450 enzymes are not stable enough for this approach. The method reported herein was developed to endogenously produce human membrane P450 proteins with a nonnative metal in the heme. This approach involved coexpression of the P450 of interest, a heme uptake system, and a chaperone in growing in iron-depleted minimal medium supplemented with the desired trans-metallated protoporphyrin. Using the steroidogenic P450 enzymes CYP17A1 and CYP21A2 and the drug-metabolizing CYP3A4, we demonstrate that this approach can be used with several human P450 enzymes and several different metals, resulting in fully folded proteins appropriate for mechanistic, functional, and structural studies including solution NMR.

摘要

人细胞色素 P450 酶是膜结合的血红素单加氧酶。与许多含血红素的酶一样,中心金属的取代对于 P450 酶的机制和结构研究是有用的。对于许多血红素蛋白,铁原卟啉辅基可以被提取并用含有另一种金属的原卟啉取代,但人膜 P450 酶不够稳定,无法采用这种方法。本文报道的方法是为了在血红素中内源产生具有非天然金属的人膜 P450 蛋白。该方法涉及在缺铁最小培养基中共同表达感兴趣的 P450、血红素摄取系统和伴侣蛋白,并用所需的转金属原卟啉补充。使用甾体生成 P450 酶 CYP17A1 和 CYP21A2 以及药物代谢 CYP3A4,我们证明该方法可用于几种人 P450 酶和几种不同的金属,从而产生完全折叠的蛋白质,适用于包括溶液 NMR 在内的机制、功能和结构研究。

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