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食品抗氧化剂的铜离子还原抗氧化能力测定:食品提取物中的维生素、多酚类和黄酮类物质

Cupric ion reducing antioxidant capacity assay for food antioxidants: vitamins, polyphenolics, and flavonoids in food extracts.

作者信息

Apak Reşat, Güçlü Kubilay, Ozyürek Mustafa, Bektas Oğlu Burcu, Bener Mustafa

机构信息

Department of Chemistry, Faculty of Engineering, Istanbul University, Istanbul, Turkey.

出版信息

Methods Mol Biol. 2008;477:163-93. doi: 10.1007/978-1-60327-517-0_14.

Abstract

Antioxidants are health beneficial compounds through their combat with reactive oxygen and nitrogen species and free radicals that may cause tissue damage leading to various diseases. This work reports the development of a simple and widely applicable antioxidant capacity index for dietary polyphenols, vitamins C and E, and plasma antioxidants utilizing the copper(II)-neocuproine (Cu(II)-Nc) reagent as the chromogenic oxidizing agent. This novel method based on an electron-transfer mechanism was named by our research group as 'cupric reducing antioxidant capacity', abbreviated as the CUPRAC method. The method is comprised of mixing the antioxidant solution with aqueous copper(II) chloride, alcoholic neocuproine, and ammonium acetate aqueous buffer at pH 7, and subsequently measuring the developed absorbance at 450 nm after 30 min. Since the color development is fast for compounds like ascorbic acid, gallic acid, and quercetin but slow for naringin and naringenin, the latter compounds are assayed after incubation at 50 degrees C on a water bath for 20 min. The flavonoid glycosides are hydrolyzed to their corresponding aglycones by refluxing in 1.2 M: HCl-containing 50% MeOH so as to exert maximal reducing power towards Cu(II)-Nc. The CUPRAC antioxidant capacities of synthetic mixtures are equal to the sum of individual capacities of antioxidant constituents, indicating lack of chemical deviations from Beer's law. Tests on antioxidant polyphenols demonstrate that the highest CUPRAC capacities are observed for epicatechin gallate, epigallocatechin gallate, quercetin, fisetin, epigallocatechin, catechin, and caffeic acid in this order, in accord with the number and position of the -OH groups as well the conjugation level of the molecule. The parallelism of the linear calibration curves of pure antioxidants in water and in a given complex matrix (plant extract) demonstrates that there are no chemical interactions of interferent nature among the solution constituents, and that the antioxidant capacities of the tested antioxidants are additive, in conformity to the Beer's law. For individual determination of ascorbic acid in fruit juices with a modified CUPRAC procedure, flavonoids are pre-extracted as their La(III) complexes prior to assay. For apricot extracts, a modified version of the CUPRAC assay based on anion exchange separation at pH 3 is applied, since sulfited-dried sample extracts contain the hydrosulfite anion interfering with the determination. For herbal tea infusions, the standard CUPRAC protocol is applied. The CUPRAC reagent is stable, easily accessible, low-cost, and is sensitive toward thiol-type antioxidants unlike FRAP. The reaction is carried out at nearly physiological pH as opposed to the acidic pH of FRAP or to the alkaline pH of Folin methods, constituting a basic advantage for the realistic assay of biological fluids.

摘要

抗氧化剂是对健康有益的化合物,它们能与活性氧、氮物种以及可能导致组织损伤并引发各种疾病的自由基作斗争。本研究报告了一种简单且广泛适用的抗氧化能力指数的开发,该指数用于测定膳食多酚、维生素C和E以及血浆抗氧化剂,使用铜(II)-新亚铜试剂(Cu(II)-Nc)作为显色氧化剂。我们的研究小组将这种基于电子转移机制的新方法命名为“铜还原抗氧化能力”,简称为CUPRAC方法。该方法包括将抗氧化剂溶液与氯化铜(II)水溶液、新亚铜灵乙醇溶液和pH为7的醋酸铵水溶液缓冲液混合,随后在30分钟后测量在450nm处产生的吸光度。由于抗坏血酸、没食子酸和槲皮素等化合物显色快,而柚皮苷和柚皮素显色慢,因此后者化合物在50℃水浴中孵育20分钟后进行测定。黄酮苷通过在含50%甲醇的1.2M盐酸中回流水解为相应的苷元,以便对Cu(II)-Nc发挥最大还原能力。合成混合物的CUPRAC抗氧化能力等于抗氧化成分各自能力之和,表明不存在与比尔定律的化学偏差。对抗氧化多酚的测试表明,表没食子儿茶素没食子酸酯、表儿茶素没食子酸酯、槲皮素、漆黄素、表儿茶素、儿茶素和咖啡酸的CUPRAC能力依次最高,这与-OH基团的数量和位置以及分子的共轭水平一致。纯抗氧化剂在水中和给定复杂基质(植物提取物)中的线性校准曲线的平行性表明,溶液成分之间不存在干扰性质的化学相互作用,并且测试的抗氧化剂的抗氧化能力是可加性的,符合比尔定律。对于用改良的CUPRAC程序单独测定果汁中的抗坏血酸,在测定前将黄酮类化合物作为其镧(III)配合物预先萃取。对于杏提取物,应用基于pH为3的阴离子交换分离的改良版CUPRAC测定法,因为亚硫酸盐干燥样品提取物中含有干扰测定的亚硫酸氢根阴离子。对于花草茶浸液,应用标准的CUPRAC方案。CUPRAC试剂稳定、易于获取、成本低,并且与FRAP不同,它对硫醇型抗氧化剂敏感。该反应在接近生理pH下进行,与FRAP的酸性pH或Folin方法的碱性pH相反,这是对生物流体进行实际测定的一个基本优势。

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