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A reliable procedure for comparison of antioxidants in rat brain homogenates.

机译:比较大鼠脑匀浆中抗氧化剂的可靠方法。

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Lipid peroxidation is a major consequence of oxidative stress and an important cause of neuronal damage in ischaemic injuries and neurodegenerative disorders such as Parkinson's disease. Recent research has focused on the development of antioxidant drugs which may delay or minimize neurodegeneration. Rapid and reliable assays are therefore necessary in order to evaluate novel antioxidant compounds. A widely adopted method for measurement of lipid peroxidation is the thiobarbituric acid reacting substances (TBARS) assay. Several variations of this method have appeared in the literature, some of which have been tested by us without success. We have therefore established a reliable procedure which takes into account the most important factors previously found to influence the TBARS method. Briefly, various concentrations of drug were added to rat brain homogenates (10% w/v in 20 mM Tris-HCl buffer, pH 7.4) and incubated at 37 degrees C for 10 min before addition of ammonium ferric sulphate (100 or 1000 microM) and a further incubation at 37 degrees C for 30 min. Proteins were then precipitated with 8.1% sodium dodecyl sulphate, the reaction stopped with 20% acetic acid, and the samples were then centrifuged for 15 min. Aliquots of supernatant were added to an equal volume of thiobarbituric acid (0.8%), samples were heated at 95 degrees C for 30 min, and then cooled on ice before reading at 532 nm. The present adaptation represents a simple and highly reproducible assay which does not require difficult extraction procedures with hazardous chemicals and results in a stable chromagen. The method has been evaluated using a number of structurally distinct antioxidants and iron chelators. IC50 values (microM) for percentage inhibition of TBARS formation were as follows: desferroxamine (1.1), U83836E (1.7), butylated hydroxytoluene (13), U74500A (20), LY231617 (22), idebenone (89), and Trolox (110). This order of potency was comparable to that found with a commercially available, but expensive kit designed to specifically measure malondialdehyde (Spearman's rank correlation coefficient, p < 0.01).
机译:脂质过氧化是氧化应激的主要结果,并且是缺血性损伤和帕金森氏病等神经退行性疾病中神经元受损的重要原因。最近的研究集中在抗氧化剂药物的开发上,该抗氧化剂可以延缓或最小化神经变性。因此,为了评估新型抗氧化剂,必须进行快速可靠的测定。脂类过氧化反应的一种广泛采用的测量方法是硫代巴比妥酸反应物质(TBARS)测定法。这种方法的几种变体已经出现在文献中,其中一些已经由我们进行了测试,但没有成功。因此,我们建立了可靠的程序,其中考虑了先前发现的影响TBARS方法的最重要因素。简而言之,将各种浓度的药物添加到大鼠脑匀浆中(在20 mM Tris-HCl缓冲液中,10%w / v,pH 7.4),并在37摄氏度下孵育10分钟,然后添加硫酸铁铵(100或1000 microM)。然后在37摄氏度下进一步孵育30分钟。然后用8.1%的十二烷基硫酸钠沉淀蛋白质,用20%的乙酸终止反应,然后将样品离心15分钟。将上清液等分试样加入等体积的硫代巴比妥酸(0.8%)中,将样品在95摄氏度下加热30分钟,然后在冰上冷却,然后在532 nm读数。本发明代表了一种简单且可高度重现的测定法,它不需要用危险化学物质进行困难的提取程序,并能产生稳定的色原。该方法已使用多种结构上不同的抗氧化剂和铁螯合剂进行了评估。抑制TBARS形成的百分比的IC50值(microM)如下:去铁胺(1.1),U83836E(1.7),丁基羟基甲苯(13),U74500A(20),LY231617(22),艾地苯醌(89)和Trolox(110) )。这种效价顺序可与市售但昂贵的试剂盒相比,后者专门设计用于测量丙二醛(Spearman等级相关系数,p <0.01)。

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