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用于测定CYP2E1催化活性的双电极策略:含细菌体的电极及6-羟基氯唑沙宗的伏安测定法

Bielectrode Strategy for Determination of CYP2E1 Catalytic Activity: Electrodes with Bactosomes and Voltammetric Determination of 6-Hydroxychlorzoxazone.

作者信息

Kuzikov Alexey V, Masamrekh Rami A, Filippova Tatiana A, Tumilovich Anastasiya M, Strushkevich Natallia V, Gilep Andrei A, Khudoklinova Yulia Yu, Shumyantseva Victoria V

机构信息

Institute of Biomedical Chemistry, 10, Pogodinskaya Street, 119121 Moscow, Russia.

Department of Biochemistry, Faculty of Biomedicine, Pirogov Russian National Research Medical University, 1, Ostrovityanova Street, 117997 Moscow, Russia.

出版信息

Biomedicines. 2024 Jan 11;12(1):152. doi: 10.3390/biomedicines12010152.

Abstract

We describe a bielectrode system for evaluation of the electrocatalytic activity of cytochrome P450 2E1 (CYP2E1) towards chlorzoxazone. One electrode of the system was employed to immobilize Bactosomes with human CYP2E1, cytochrome P450 reductase (CPR), and cytochrome (cyt ). The second electrode was used to quantify CYP2E1-produced 6-hydroxychlorzoxazone by its direct electrochemical oxidation, registered using square-wave voltammetry. Using this system, we determined the steady-state kinetic parameters of chlorzoxazone hydroxylation by CYP2E1 of Bactosomes immobilized on the electrode: the maximal reaction rate () was 1.64 ± 0.08 min, and the Michaelis constant () was 78 ± 9 μM. We studied the electrochemical characteristics of immobilized Bactosomes and have revealed that electron transfer from the electrode occurs both to the flavin prosthetic groups of CPR and the heme iron ions of CYP2E1 and cyt . Additionally, it has been demonstrated that CPR has the capacity to activate CYP2E1 electrocatalytic activity towards chlorzoxazone, likely through intermolecular electron transfer from the electrochemically reduced form of CPR to the CYP2E1 heme iron ion.

摘要

我们描述了一种用于评估细胞色素P450 2E1(CYP2E1)对氯唑沙宗电催化活性的双电极系统。该系统的一个电极用于固定含有人类CYP2E1、细胞色素P450还原酶(CPR)和细胞色素c(cyt c)的细菌体。第二个电极用于通过其直接电化学氧化来定量CYP2E1产生的6-羟基氯唑沙宗,使用方波伏安法进行记录。利用该系统,我们测定了固定在电极上的细菌体中CYP2E1对氯唑沙宗羟基化的稳态动力学参数:最大反应速率(Vmax)为1.64±0.08 min⁻¹,米氏常数(Km)为78±9 μM。我们研究了固定化细菌体的电化学特性,发现电子从电极转移到CPR的黄素辅基以及CYP2E1和cyt c的血红素铁离子上。此外,已经证明CPR能够激活CYP2E1对氯唑沙宗的电催化活性,可能是通过从CPR的电化学还原形式向CYP2E1血红素铁离子的分子间电子转移。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2d92/10812958/43cfc8603681/biomedicines-12-00152-sch001.jpg

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