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利用黄嘌呤氧化酶和次黄嘌呤测定法分析超氧化物引起的二羟乙基啶荧光动力学。

Analysis of kinetics of dihydroethidium fluorescence with superoxide using xanthine oxidase and hypoxanthine assay.

机构信息

Department of Biomedical Engineering, Wayne State University, 5050 Anthony Wayne Dr., Detroit, MI 48202, USA.

出版信息

Ann Biomed Eng. 2013 Feb;41(2):327-37. doi: 10.1007/s10439-012-0653-x. Epub 2012 Sep 11.

DOI:10.1007/s10439-012-0653-x
PMID:22965641
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3544990/
Abstract

Superoxide (O(2) (-)) is an important reactive oxygen species (ROS), and has an essential role in physiology and pathophysiology. An accurate detection of O(2) (-) is needed to better understand numerous vascular pathologies. In this study, we performed a mechanistic study by using the xanthine oxidase (XOD)/hypoxanthine (HX) assay for O(2) (-) generation and a O(2) (-) sensitive fluorescent dye dihydroethidium (DHE) for O(2) (-) measurement. To quantify O(2) (-) and DHE interactions, we measured fluorescence using a microplate reader. We conducted a detailed reaction kinetic analysis for DHE-O(2) (-) interaction to understand the effect of O(2) (-) self-dismutation and to quantify DHE-O(2) (-) reaction rate. Fluorescence of DHE and 2-hydroethidium (EOH), a product of DHE and O(2) (-) interaction, were dependent on reaction conditions. Kinetic analysis resulted in a reaction rate constant of 2.169 ± 0.059 × 10(3) M(-1) s(-1) for DHE-O(2) (-) reaction that is ~100× slower than the reported value of 2.6 ± 0.6 × 10(5) M(-1) s(-1). In addition, the O(2) (-) self-dismutation has significant effect on DHE-O(2) (-) interaction. A slower reaction rate of DHE with O(2) (-) is more reasonable for O(2) (-) measurements. In this manner, the DHE is not competing with superoxide dismutase and NO for O(2) (-). Results suggest that an accurate measurement of O(2) (-) production rate may be difficult due to competitive interference for many factors; however O(2) (-) concentration may be quantified.

摘要

超氧阴离子(O(2) (-))是一种重要的活性氧物质(ROS),在生理和病理生理学中具有重要作用。为了更好地理解许多血管病理学,需要准确检测 O(2) (-)。在这项研究中,我们通过黄嘌呤氧化酶(XOD)/次黄嘌呤(HX)测定法进行 O(2) (-)生成的机制研究,并使用超氧阴离子敏感荧光染料二氢乙啶(DHE)进行 O(2) (-)测量。为了定量 O(2) (-)和 DHE 的相互作用,我们使用微孔板读数器测量荧光。我们对 DHE-O(2) (-)相互作用进行了详细的反应动力学分析,以了解 O(2) (-)自歧化的影响,并定量 DHE-O(2) (-)反应速率。DHE 和 2-羟乙基啶(EOH)的荧光,DHE 和 O(2) (-)相互作用的产物,依赖于反应条件。动力学分析得到 DHE-O(2) (-)反应的反应速率常数为 2.169 ± 0.059 × 10(3) M(-1) s(-1),这比报道的值 2.6 ± 0.6 × 10(5) M(-1) s(-1)慢约 100 倍。此外,O(2) (-)的自歧化对 DHE-O(2) (-)相互作用有显著影响。DHE 与 O(2) (-)的反应速率较慢,更有利于 O(2) (-)的测量。以这种方式,DHE 不会与超氧化物歧化酶和 NO 竞争 O(2) (-)。结果表明,由于许多因素的竞争干扰,准确测量 O(2) (-)生成速率可能很困难;但是可以定量 O(2) (-)浓度。

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