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超氧化物与三苯甲基自由基的反应:对分光光度法测定超氧化物的意义。

Reaction of superoxide with trityl radical: implications for the determination of superoxide by spectrophotometry.

作者信息

Kutala Vijay Kumar, Parinandi Narasimham L, Zweier Jay L, Kuppusamy Periannan

机构信息

Center for Biomedical EPR Spectroscopy and Imaging, Department of Internal Medicine, Davis Heart and Lung Research Institute, Ohio State University, Columbus, OH, USA.

出版信息

Arch Biochem Biophys. 2004 Apr 1;424(1):81-8. doi: 10.1016/j.abb.2004.01.020.

Abstract

Superoxide radicals can be measured by redox methods which utilize the oxidation/reduction reactions of specific compounds. The redox methods, however, suffer from various interferences, which limit their use in the assay of superoxide. Electron paramagnetic resonance (EPR) spectroscopy using spin traps has been widely used as an alternative and direct technique to measure superoxide radicals. In our recent study, we have demonstrated the detection of superoxide in cellular system by EPR spectroscopy with triarylmethyl (trityl) free radical, TAM Ox063. TAM is highly water-soluble and stable in the presence of many biological oxidizing and reducing agents such as hydrogen peroxide, ascorbate, and glutathione. TAM reacts with superoxide with an apparent second order rate constant of 3.1x10(3)M(-1)s(-1). In the present work, we investigated the feasibility of a spectrophotometric assay of superoxide by taking advantage of the newly formed distinct absorption peak corresponding to the product formed from the reaction between TAM and superoxide. The effects of different fluxes of superoxide and concentrations of TAM on the efficiency and sensitivity of quantification of superoxide were investigated and compared with the widely used cytochrome c method of superoxide determination. The results demonstrated that the TAM method is comparable to the cytochrome c method for the assay of superoxide and further revealed that the assay is not affected by the presence of hydrogen peroxide. In summary, the TAM spectrophotometric assay of superoxide provides a suitable alternative method to the cytochrome c assay to measure superoxide and further complements our earlier reported TAM-EPR assay of superoxide.

摘要

超氧阴离子自由基可以通过利用特定化合物氧化/还原反应的氧化还原方法来测定。然而,这些氧化还原方法存在各种干扰,这限制了它们在超氧阴离子测定中的应用。使用自旋捕获剂的电子顺磁共振(EPR)光谱已被广泛用作测量超氧阴离子自由基的替代直接技术。在我们最近的研究中,我们已经证明通过使用三芳基甲基(三苯甲基)自由基TAM Ox063的EPR光谱在细胞系统中检测超氧阴离子。TAM具有高度水溶性,并且在许多生物氧化和还原剂如过氧化氢、抗坏血酸盐和谷胱甘肽存在下稳定。TAM与超氧阴离子反应的表观二级速率常数为3.1x10(3)M(-1)s(-1)。在本工作中,我们利用TAM与超氧阴离子反应形成的产物对应的新形成的独特吸收峰,研究了超氧阴离子分光光度测定法的可行性。研究了不同超氧阴离子通量和TAM浓度对超氧阴离子定量效率和灵敏度的影响,并与广泛使用的细胞色素c超氧阴离子测定方法进行了比较。结果表明,TAM方法在超氧阴离子测定方面与细胞色素c方法相当,并且进一步表明该测定不受过氧化氢存在的影响。总之,超氧阴离子的TAM分光光度测定法为细胞色素c测定法提供了一种合适的替代方法来测量超氧阴离子,并且进一步补充了我们早期报道的超氧阴离子的TAM-EPR测定法。

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