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谷胱甘肽过氧化物酶抑制法测定柴油机废气和烟草烟雾中的亲电污染物。

Glutathione peroxidase inhibitory assay for electrophilic pollutants in diesel exhaust and tobacco smoke.

机构信息

Department of Epidemiology, School of Medicine, University of California, Irvine, CA 92697, USA.

出版信息

Anal Bioanal Chem. 2012 Apr;403(2):431-41. doi: 10.1007/s00216-012-5823-z. Epub 2012 Feb 21.

Abstract

We developed a rapid kinetic bioassay demonstrating the inhibition of glutathione peroxidase 1 (GPx-1) by organic electrophilic pollutants, such as acrolein, crotonaldehyde, and p-benzoquinone, that are frequently found as components of tobacco smoke, diesel exhaust, and other combustion sources. In a complementary approach, we applied a high-resolution proton-transfer reaction time-of-flight mass spectrometer to monitor in real-time the generation of electrophilic volatile carbonyls in cigarette smoke. The new bioassay uses the important antioxidant selenoenzyme GPx-1, immobilized to 96-well microtiter plates, as a probe. The selenocysteine bearing subunits of the enzyme's catalytic site are viewed as cysteine analogues and are vulnerable to electrophilic attack by compounds with conjugated carbonyl systems. The immobilization of GPx-1 to microtiter plate wells enabled facile removal of excess reactive inhibitory compounds after incubation with electrophilic chemicals or aqueous extracts of air samples derived from different sources. The inhibitory response of cigarette smoke and diesel exhaust particle extracts were compared with chemical standards of a group of electrophilic carbonyls and the arylating p-benzoquinone. GPx-1 activity was directly inactivated by millimolar concentrations of highly reactive electrophilic chemicals (including acrolein, glyoxal, methylglyoxal, and p-benzoquinone) and extracts of diesel and cigarette smoke. We conclude that the potential of air pollutant components to generate oxidative stress may be, in part, a result of electrophile-derived covalent modifications of enzymes involved in the cytosolic antioxidant defense.

摘要

我们开发了一种快速动力学生物测定法,用于证明谷胱甘肽过氧化物酶 1(GPx-1)被有机亲电污染物(如丙烯醛、巴豆醛和对苯醌)抑制,这些污染物经常作为烟草烟雾、柴油尾气和其他燃烧源的成分存在。在一种互补的方法中,我们应用高分辨率质子转移反应飞行时间质谱仪实时监测香烟烟雾中亲电挥发性羰基化合物的生成。新的生物测定法使用重要的抗氧化硒酶 GPx-1,固定在 96 孔微量滴定板上,作为探针。酶催化部位的硒半胱氨酸亚基被视为半胱氨酸类似物,容易受到具有共轭羰基系统的化合物的亲电攻击。GPx-1 固定在微量滴定板孔中,便于在与亲电化学物质或来自不同来源的空气样品的水提取物孵育后去除多余的反应性抑制化合物。香烟烟雾和柴油尾气颗粒提取物的抑制反应与一组亲电羰基化合物和芳族对苯醌的化学标准进行了比较。毫摩尔浓度的高反应亲电化学物质(包括丙烯醛、乙二醛、甲基乙二醛和对苯醌)和柴油及香烟烟雾提取物直接使 GPx-1 失活。我们得出结论,空气污染物成分产生氧化应激的潜力可能部分是由于细胞溶质抗氧化防御中涉及的酶的亲电衍生共价修饰所致。

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