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Development and Evaluation of Kinetic Spectrophotometric Assays for Horseradish Peroxidase by Catalytic Coupling of Paraphenylenediamine and Mequinol

机译:对苯二胺与对苯二酚催化偶合动力学分析光度法测定辣根过氧化物酶

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摘要

This paper presents a novel spectrophotometric method to measure peroxidase activity using paraphenylenediamine dihydrochloride (PPDD) and Mequinol (MQ). The PPDD traps the free radical, and gets oxidized to electrophilic 1,4-diimine; this couples with MQ to an give intense violet-colored chromogenic species with the maximum absorbance at 560 nm. This assay was adopted for the quantification of hydrogen peroxide between 10 x 10(-6) to 80 x 10(-6) M. From the kinetic data, a two-substrate ping-pong mechanism of peroxidase was established. Catalytic efficiency and catalytic power of commercial peroxidase were 0.204 x 10(6) M(-1) min(-1) and 2.86 x 10(-4) min(-1), respectively. The catalytic constant (k(cat)) of the proposed method was 0.2080 x 10(3) min(-1). As a simple, rapid, precise and sensitive technique, PPDD-MQ stands as a potential replacement for the traditional guaiacol method. Applications to the plant extracts increase its relevance in the field of biochemical analysis.
机译:本文提出了一种新的分光光度法,使用对苯二胺二盐酸盐(PPDD)和甲基喹啉(MQ)测定过氧化物酶活性。 PPDD捕获自由基,并被氧化为亲电子的1,4-二亚胺;这与MQ结合可产生强烈的紫色生色物质,在560 nm处具有最大吸光度。此测定法用于定量10 x 10(-6)至80 x 10(-6)M之间的过氧化氢。根据动力学数据,建立了过氧化物酶的两底物乒乓机制。商业过氧化物酶的催化效率和催化能力分别为0.204 x 10(6)M(-1)min(-1)和2.86 x 10(-4)min(-1)。该方法的催化常数(k(cat))为0.2080 x 10(3)min(-1)。作为一种简单,快速,精确和灵敏的技术,PPDD-MQ可以替代传统的愈创木酚方法。在植物提取物中的应用增加了其在生化分析领域中的相关性。

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