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首页> 外文期刊>Analytical Letters >Novel Iron(III)-Induced Prooxidant Activity Measurement Using a Solid Protein Sensor in Comparison with a Copper(II)-Induced Assay
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Novel Iron(III)-Induced Prooxidant Activity Measurement Using a Solid Protein Sensor in Comparison with a Copper(II)-Induced Assay

机译:新颖的铁(III) - 与铜(II)诱导的测定相比,使用固体蛋白传感器诱导引发活性测量

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摘要

The iron(III) and Cu(II) reducing ability of common antioxidants may be an indirect measure of their prooxidant activity, because the reduced ions may generate reactive oxygen species (ROS). This study aimed to develop a new Fe(III)-ferrozine spectrophotometric prooxidant activity assay using a protein-based solid biosensor prepared from Ca(II) and chicken egg whites. This new assay involved the reduction of Fe(III) ions to Fe(II) by antioxidant compounds and the binding of the formed Fe(II) to the solid biosensor. As an indicator of the prooxidant activity of antioxidants on proteins, the protein-bound Fe(II) was colorimetrically determined with ferrozine at 562 nm. The prooxidant activities of antioxidant compounds such as gallic acid, catechin, epicatechin, epigallocatechin gallate, and chlorogenic acid were determined across a wide range of final concentrations between 0.25 and 2500 μM. Most of the tested compounds showed prooxidant activity above a concentration of 2.50 μM with the Fe(III)-based method. In addition, the findings of the new method were compared with those of the modified Cu(II)ňeocuproine (Nc) method previously developed by the same authors based on the principle of copper(II) reduction by antioxidants in the presence of a Ca(II)-proteinate sensor.
机译:常见抗氧化剂的铁(III)和Cu(II)可以是其寄生活性的间接测量,因为还原离子可能产生反应性氧(ROS)。该研究旨在使用由Ca(II)和鸡蛋白酸盐制备的蛋白质的固体生物传感器来开发新的Fe(III) - 氧化丁分光光度分光光度法促体活性测定。该新测定涉及通过抗氧化剂化合物和所形成的Fe(II)与固体生物传感器的结合减少Fe(III)离子的Fe(II)。作为蛋白质抗氧化剂的促氧化剂活性的指示,蛋白质结合的Fe(II)用562nm的铁嗪进行比例测定。在0.25-2500μm之间的宽范围的最终浓度下测定抗氧化剂化合物如食子酸,儿茶素,表皮素,表皮酰胺和鲜成酸的过约氧化物的活性。大多数经测试的化合物显示出浓度为2.50μm的过约活性,得到Fe(III)的方法。此外,将新方法的发现与先前由同一作者的改性Cu(II)ň欧普洛汀(NC)方法的方法进行比较,基于通过抗氧化剂在CA( ii) - 蛋白质传感器。

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