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蛋白质的体外臭氧暴露。

In vitro exposure of proteins to ozone.

机构信息

Department of Pediatrics, The Pennsylvania State University College of Medicine, Hershey, PennsylvaniaUSA.

出版信息

Toxicol Mech Methods. 2002;12(1):1-16. doi: 10.1080/15376510209167932.

Abstract

An in vitro system has been developed to expose proteins to ozone. The system is designed to deliver consistent and accurate levels of ozone over a range of concentrations (between 0.1 and >/=10 ppm) with extended exposure times (24 h or longer) in a humidified environment (100%). In the experiment presented in this article, ozone concentrations between 0.1 and 2.0 ppm were used. Ozone was generated by an electrical discharge ozonizer to ensure stability; it was continually monitored by an ultraviolet ozone analyzer and was precisely controlled by mass flow controllers, which gave reproducible results between runs. Humidity was closely regulated in the system to allow small amounts of protein solutions (50 muL or less) to be exposed without significant changes (<0.2%) in sample volume. The degree of surfactant protein-A (SP-A) oxidation by ozone was measured between runs to demonstrate the reproducibility of the system. A detailed description of the system is given, and protein oxidation detection methods and their limitations are discussed. Using these methods, we were able to assess oxidation of SP-A that apparently occurred prior to its isolation from the lung by bronchoalveolar lavage. This in vitro system allowed us to expose small amounts of protein to ozone in a simple, highly controlled, and reproducible manner.

摘要

已经开发出一种体外系统来使蛋白质暴露于臭氧中。该系统旨在提供一致且准确的臭氧浓度(0.1 至>/=10 ppm 之间),并在加湿环境(100%)中进行长时间(24 小时或更长时间)暴露。在本文介绍的实验中,使用了 0.1 至 2.0 ppm 的臭氧浓度。通过电晕放电臭氧发生器产生臭氧以确保稳定性;通过紫外线臭氧分析仪连续监测,并通过质量流量控制器精确控制,在运行之间可获得可重复的结果。该系统对湿度进行了严格控制,允许对少量蛋白质溶液(50 μL 或更少)进行暴露,而样品体积没有明显变化(<0.2%)。在运行之间测量表面活性剂蛋白-A(SP-A)的臭氧氧化程度,以证明该系统的重现性。详细描述了该系统,并讨论了蛋白质氧化检测方法及其局限性。使用这些方法,我们能够评估在通过支气管肺泡灌洗从肺部分离之前,SP-A 显然发生的氧化。该体外系统允许我们以简单、高度控制和可重复的方式使少量蛋白质暴露于臭氧中。

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