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Comparison of Mitochondrial Superoxide Detection Ex Vivo/In Vivo by mitoSOX HPLC Method with Classical Assays in Three Different Animal Models of Oxidative Stress

机译:在三种不同的氧化应激动物模型中使用mitoSOX HPLC方法与经典方法对体内线粒体超氧化物检测的体内/体外比较

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摘要

Background: Reactive oxygen and nitrogen species (RONS such as H O , nitric oxide) are generated within the organism. Whereas physiological formation rates confer redox regulation of essential cellular functions and provide the basis for adaptive stress responses, their excessive formation contributes to impaired cellular function or even cell death, organ dysfunction and severe disease phenotypes of the entire organism. Therefore, quantification of RONS formation and knowledge of their tissue/cell/compartment-specific distribution is of great biological and clinical importance. Methods: Here, we used a high-performance/pressure liquid chromatography (HPLC) assay to quantify the superoxide-specific oxidation product of the mitochondria-targeted fluorescence dye triphenylphosphonium-linked hydroethidium (mitoSOX) in biochemical systems and three animal models with established oxidative stress. Type 1 diabetes (single injection of streptozotocin), hypertension (infusion of angiotensin-II for 7 days) and nitrate tolerance (infusion of nitroglycerin for 4 days) was induced in male Wistar rats. Results: The usefulness of mitoSOX/HPLC for quantification of mitochondrial superoxide was confirmed by xanthine oxidase activity as well as isolated stimulated rat heart mitochondria in the presence or absence of superoxide scavengers. Vascular function was assessed by isometric tension methodology and was impaired in the rat models of oxidative stress. Vascular dysfunction correlated with increased mitoSOX oxidation but also classical RONS detection assays as well as typical markers of oxidative stress. Conclusion: mitoSOX/HPLC represents a valid method for detection of mitochondrial superoxide formation in tissues of different animal disease models and correlates well with functional parameters and other markers of oxidative stress.
机译:背景:生物体内会产生活性氧和氮物质(RONS,例如H O,一氧化氮)。生理形成速率赋予氧化还原调节基本的细胞功能,并为适应性应激反应提供基础,而它们的过度形成则导致整个有机体的细胞功能受损甚至细胞死亡,器官功能障碍和严重的疾病表型。因此,量化RONS的形成及其组织/细胞/隔室特异性分布的知识具有重要的生物学和临床意义。方法:在这里,我们使用了高性能/高压液相色谱(HPLC)分析法,定量了生化系统中线粒体靶向的荧光染料三苯基hydro连接的氢乙啶(mitoSOX)的超氧化物特异性氧化产物和建立了氧化性的三个动物模型。强调。在雄性Wistar大鼠中诱发1型糖尿病(单次注射链脲佐菌素),高血压(输注血管紧张素II 7天)和硝酸盐耐受性(输注硝酸甘油4天)。结果:通过黄嘌呤氧化酶活性以及在存在或不存在超氧化物清除剂的情况下分离的刺激的大鼠心脏线粒体,证实了mitoSOX / HPLC对定量线粒体超氧化物的有用性。通过等轴测张力方法评估了血管功能,并且在大鼠氧化应激模型中受损。血管功能障碍与mitoSOX氧化增加有关,而且与经典RONS检测方法以及氧化应激的典型标志物有关。结论:mitoSOX / HPLC是检测不同动物疾病模型组织中线粒体超氧化物形成的有效方法,并且与功能参数和其他氧化应激标记物具有良好的相关性。

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