虹鳟鱼肝细胞活性氧的荧光动力学研究。

M. Yazdani, K. Hylland
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引用次数: 1

摘要

采用5-,6-氯甲基-2',7'-二氯二氢荧光素(CM-H2DCFDA)、二氢霍达明123 (DHR 123)和二氢乙啶(DHE)三种荧光探针研究了虹鳟鱼肝细胞原代培养中活性氧(ROS)形成的动力学。细胞培养分别装载三种探针。然后将肝细胞暴露于无血清Leibovitz培养基中的Cu (0.15-10 mM)中30分钟,然后在30分钟内用荧光板阅读器定量。使用荧光探针5-羧基荧光素二乙酸乙酯-乙酰氧基甲酯(CFDA-AM)和单氯比烷定量膜完整性和谷胱甘肽(GSH)含量。CM-H2DCFDA显示,随着Cu浓度的增加,ROS的形成增加,而DHR 123的荧光减弱。在两种探针的最高浓度(2.5 mM和10 mM)下,对照组和治疗组之间存在显著差异。DHE荧光低于其他两种探针,并且似乎不受任何暴露的影响。此外,GSH的消耗和膜完整性随着Cu浓度的增加呈剂量依赖性,在2.5 mM和10 mM两个终点均观察到显著影响。结果表明,CMH2DCFDA和DHR 123在鳟鱼肝细胞中检测到其靶cu诱导的ROS的发展,但其方式相反。发现DHE不适合用于检测该模型系统中ROS形成的动力学。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A Kinetic Study of Reactive Oxygen Species in Rainbow Trout Hepatocytes by Fluorometry.
The kinetics of reactive oxygen species (ROS) formation in a primary culture of rainbow trout hepatocytes was investigated using three fluorescent probes: 5-,6-chloromethyl-2',7'-dichlorodihydrofluorescein diacetate (CM-H2DCFDA), dihydrorhodamine 123 (DHR 123), and dihydroethidium (DHE). The cell cultures were loaded with the three probes, separately. Hepatocytes were then exposed to Cu (0.15-10 mM) in serum-free Leibovitz's medium for 30 min before being quantified by a fluorescence plate reader during 30 min. Membrane integrity and glutathione (GSH) content were quantified using the fluorescent probes 5-carboxyfluorescein diacetate-acetoxymethyl ester (CFDA-AM) and monochlorobimane. Increasing ROS formation with increasing concentrations of Cu was shown using CM-H2DCFDA, whereas DHR 123 fluorescence decreased. Significant differences between control and treatment groups were observed at the highest concentrations (2.5 and 10 mM) for both probes. DHE fluorescence was lower than that of the other two probes and did not appear to be affected by any exposure. Additionally, a dose-dependent depletion of GSH and decreasing membrane integrity with increasing Cu concentrations were demonstrated, with significant effects observed at 2.5 and 10 mM for both endpoints. The results showed that both CMH2DCFDA and DHR 123 detected the development of their target Cu-induced ROS in trout hepatocytes but did so in opposite fashions. DHE was found to be unsuitable for detecting kinetics of ROS formation in this model system.
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