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基于双缩脲反应,开发一种使用铜螯合剂铬天青B的蛋白质测定方法。

Development of a protein assay with copper chelator chromeazurol B, based on the biuret reaction.

作者信息

Hokazono Eisaku, Ota Eri, Goto Taiki, Fukumoto Saori, Kayamori Yuzo, Uchiumi Takeshi, Osawa Susumu

机构信息

Division of Biological Science and Technology Department of Health Sciences, Graduate School of Medical Sciences, Kyushu University, Japan.

Division of Biological Science and Technology Department of Health Sciences, Graduate School of Medical Sciences, Kyushu University, Japan; Research Center for Micro Blood Analysis, Leisure, Inc., Japan.

出版信息

Anal Biochem. 2021 Oct 1;630:114320. doi: 10.1016/j.ab.2021.114320. Epub 2021 Jul 31.

Abstract

This study aimed to provide a novel and highly sensitive protein assay based on the biuret reaction and using chromeazurol B, a metal chelate compound. The method consists of two reagents and an automated analyzer. First, a complex of copper and protein (biuret reaction) is formed. Second, a chelating reagent containing chromeazurol B forms a three-dimensional complex of protein, copper, and chromeazurol B at neutral pH, resulting in highly sensitive coloration. The intra-assay (n = 20) variation for the three levels was 3.54 % or lower at each concentration. Each response with α, β-, and γ-globulin was 103.8 % and 104.3 %, respectively, against albumin. The molar absorption coefficient (ε) of the present method was 2.5 × 10 m/mol against human albumin, higher than that of the commercially available Lowry method (ε = 8.7 × 10 m/mol), which is based on the same principle. The correlation test for the pyrogallol method with 30 urine samples showed good performance (r = 0.961). The method described here (the Biuret-based CAB method) is a more sensitive and rapid assay than the Lowry method, and it may also be applied to biological samples because of its similar reactivity towards various proteins.

摘要

本研究旨在基于双缩脲反应并使用金属螯合物铬天青B提供一种新型且高灵敏度的蛋白质检测方法。该方法由两种试剂和一台自动分析仪组成。首先,形成铜与蛋白质的复合物(双缩脲反应)。其次,含铬天青B的螯合试剂在中性pH条件下形成蛋白质、铜和铬天青B的三维复合物,从而产生高灵敏度的显色反应。在每个浓度下,三个水平的批内(n = 20)变异为3.54%或更低。α、β - 和γ球蛋白相对于白蛋白的每个响应分别为103.8%和104.3%。本方法针对人白蛋白的摩尔吸收系数(ε)为2.5×10 m/mol,高于基于相同原理的市售洛氏法(ε = 8.7×10 m/mol)。对30份尿液样本进行的邻苯三酚法相关性测试显示性能良好(r = 0.961)。此处所述的方法(基于双缩脲的CAB法)是一种比洛氏法更灵敏、更快速的检测方法,并且由于其对各种蛋白质具有相似的反应性,也可应用于生物样本。

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