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基于苏木精自氧化的超氧化物歧化酶阴性和阳性检测

Negative and positive assays of superoxide dismutase based on hematoxylin autoxidation.

作者信息

Martin J P, Dailey M, Sugarman E

出版信息

Arch Biochem Biophys. 1987 Jun;255(2):329-36. doi: 10.1016/0003-9861(87)90400-0.

Abstract

Hematoxylin, a natural dye commonly used as a histological stain, generates superoxide upon oxidation to its quinonoid product, hematein. The parameters affecting this reaction were assessed in developing a new and versatile assay for superoxide dismutase. The autoxidation of hematoxylin to hematein was accompanied by an increase in absorbance between 400 and 670 nm. The autoxidation rate was proportional to hematoxylin concentration and increased with pH above 6.55. Trace metals accelerated the autoxidation and this effect was eliminated by EDTA. Superoxide dismutase inhibited the autoxidation 90-95% below pH 7.8, but above pH 8.1 the rate was augmented by superoxide dismutase. The rate inhibition at low pH was proportional to the superoxide dismutase concentration up to 70% inhibition. The rate acceleration at high pH was proportional to superoxide dismutase concentration up to approximately 200% acceleration. The autoxidation rate was not significantly affected by ethanol, cyanide, azide, hydrogen peroxide, or catalase. However, the reaction was inhibited by the reducing agents NADH, reduced glutathione, ascorbate, and dithiothreitol, and by undialyzed extracts of Escherichia coli B. When cell extracts were dialyzed prior to assay, the degree of inhibition observed was proportional to the concentration of superoxide dismutase in the extract. These observations form the basis for negative and positive assays of superoxide dismutase which are inexpensive and simple to perform. The negative assay has the added advantage of being applicable at physiological pH.

摘要

苏木精是一种常用作组织学染色剂的天然染料,氧化成其醌类产物苏木色精时会产生超氧化物。在开发一种新的通用超氧化物歧化酶测定方法时,对影响该反应的参数进行了评估。苏木精自氧化成苏木色精的过程中,在400至670纳米之间吸光度增加。自氧化速率与苏木精浓度成正比,在pH高于6.55时随pH升高而增加。痕量金属加速自氧化,而这种效应可被乙二胺四乙酸消除。在pH 7.8以下,超氧化物歧化酶抑制自氧化90%至95%,但在pH 8.1以上,超氧化物歧化酶会提高反应速率。低pH下的速率抑制与超氧化物歧化酶浓度成正比,最高可达70%抑制率。高pH下的速率加速与超氧化物歧化酶浓度成正比,最高可达约200%的加速率。自氧化速率不受乙醇、氰化物、叠氮化物、过氧化氢或过氧化氢酶的显著影响。然而,该反应受到还原剂烟酰胺腺嘌呤二核苷酸(NADH)、还原型谷胱甘肽、抗坏血酸和二硫苏糖醇以及大肠杆菌B未透析提取物的抑制。当在测定前对细胞提取物进行透析时,观察到的抑制程度与提取物中超氧化物歧化酶的浓度成正比。这些观察结果构成了超氧化物歧化酶阴性和阳性测定的基础,这些测定方法成本低廉且操作简单。阴性测定的额外优点是可在生理pH下应用。

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