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超氧化物歧化酶活性检测方法的重新评估及试剂盒的建立。

Reevaluation of assay methods and establishment of kit for superoxide dismutase activity.

作者信息

Oyanagui Y

出版信息

Anal Biochem. 1984 Nov 1;142(2):290-6. doi: 10.1016/0003-2697(84)90467-6.

Abstract

Superoxide dismutase (SOD) activity was measured by seven assay methods. The nitrite method was found to be the best for our SOD assay kit. This method was then modified to give better sensitivity and minimize interference by coexisting protein, a factor which has been previously ignored. Hydroxylamine or its O-sulfonic acid, xanthine oxidase, hypoxanthine, EDTA, and the sample were incubated with or without KCN at pH 8.2, 37 degrees C, for 30 min. Diazo dye-forming reagent was added and the absorption was measured at 550 nm. Human plasma and erythrocyte lysate from healthy adults and Down's syndrome patients were assayed by this SOD kit and by the cytochrome c method. Our kit gave 8.5 times higher sensitivity than the cytochrome c method. This high sensitivity allowed the use of a simple spectrophotometer and, moreover, only one dilution was needed to determine the SOD unit with the help of our formulas. Good recovery, reproducibility, and stability of reagents were demonstrated.

摘要

采用七种测定方法测定超氧化物歧化酶(SOD)活性。发现亚硝酸盐法最适合我们的SOD检测试剂盒。随后对该方法进行了改进,以提高灵敏度并最大限度地减少共存蛋白质的干扰,而这一因素此前一直被忽视。在pH 8.2、37℃条件下,将羟胺或其O -磺酸、黄嘌呤氧化酶、次黄嘌呤、乙二胺四乙酸(EDTA)和样品与或不与氰化钾一起孵育30分钟。加入重氮染料形成试剂,并在550nm处测量吸光度。使用该SOD试剂盒和细胞色素c法对健康成年人及唐氏综合征患者的人血浆和红细胞裂解物进行检测。我们的试剂盒灵敏度比细胞色素c法高8.5倍。这种高灵敏度使得可以使用简单的分光光度计,此外,借助我们的公式,只需进行一次稀释就能确定SOD单位。结果表明该试剂盒具有良好的回收率、重现性和试剂稳定性。

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