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通过比色筛选法鉴定人含黄素单加氧酶3底物

Identification of human flavin-containing monooxygenase 3 substrates by a colorimetric screening assay.

作者信息

Catucci Gianluca, Polignano Isabelle, Cusumano Debora, Medana Claudio, Gilardi Gianfranco, Sadeghi Sheila J

机构信息

Department of Life Sciences and Systems Biology, University of Torino, 10123 Turin, Italy.

Department of Molecular Biotechnology and Health Sciences, University of Torino, 10125 Turin, Italy.

出版信息

Anal Biochem. 2017 Apr 1;522:46-52. doi: 10.1016/j.ab.2017.01.024. Epub 2017 Jan 27.

DOI:10.1016/j.ab.2017.01.024
PMID:28137602
Abstract

Human hepatic flavin-containing monooxygenase 3 is a phase I drug-metabolizing enzyme that is responsible for the oxidation of a variety of drugs and xenobiotics. This work reports on a high throughput rapid colorimetric assay for the screening of substrates or inhibitors of this enzyme. The method is based on the competition of two substrates for access to the active site of hFMO3 whereby the enzymatic product of the first drug converts nitro-5-thiobenzoate (TNB, yellow) to 5,5'-dithiobis (2-nitrobenzoate) (DTNB, colourless). Upon addition of a competing substrate, the amount of detected DNTB is decreased. The assay is validated testing three known substrates of hFMO3, namely benzydamine, tozasertib and tamoxifen. The latter drugs resulted in 41%-55% inhibition. In addition, two other drugs also classified as doping drugs, selegiline and clomiphene, were selected based on their chemical structure similarity to known substrates of hFMO3. These drugs showed 21% and 60% inhibition in the colorimetric assay and therefore were proven to be hFMO3 substrates. LC-MS was used to confirm their N-oxide products. Further characterisation of these newly identified hFMO3 substrates was performed determining their K and k values that resulted to be 314 μM and 1.4 min for selegiline and, 18 μM and 0.1 min for clomiphene. This method paves the way for a rapid automated high throughput screening of nitrogen-containing compounds as substrates/inhibitors of hFMO3.

摘要

人肝含黄素单加氧酶3是一种I相药物代谢酶,负责多种药物和外源性物质的氧化。这项工作报道了一种用于筛选该酶底物或抑制剂的高通量快速比色测定法。该方法基于两种底物竞争进入hFMO3活性位点,其中第一种药物的酶促产物将硝基-5-硫代苯甲酸酯(TNB,黄色)转化为5,5'-二硫代双(2-硝基苯甲酸酯)(DTNB,无色)。加入竞争性底物后,检测到的DNTB量减少。通过测试hFMO3的三种已知底物,即苄达明、托扎替布和他莫昔芬,对该测定法进行了验证。后两种药物导致41%-55%的抑制率。此外,根据与hFMO3已知底物的化学结构相似性,选择了另外两种也被归类为兴奋剂的药物,即司来吉兰和氯米芬。这些药物在比色测定中显示出21%和60%的抑制率,因此被证明是hFMO3底物。采用LC-MS确认了它们的N-氧化物产物。对这些新鉴定的hFMO3底物进行了进一步表征,测定了它们的K和k值,司来吉兰的K和k值分别为314μM和1.4分钟,氯米芬的K和k值分别为18μM和0.1分钟。该方法为快速自动化高通量筛选含氮化合物作为hFMO3的底物/抑制剂铺平了道路。

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