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用于癌胚抗原快速免分离免疫分析的新型安培免疫传感器。

Novel amperometric immunosensor for rapid separation-free immunoassay of carcinoembryonic antigen.

作者信息

Dai Zong, Yan Feng, Yu Hua, Hu Xiaoya, Ju Huangxian

机构信息

Department of Chemistry, Institute of Analytical Science, State Key Laboratory of Coordination Chemistry, Nanjing University, Hankou Lu, Nanjing 210093, PR China.

出版信息

J Immunol Methods. 2004 Apr;287(1-2):13-20. doi: 10.1016/j.jim.2004.01.012.

Abstract

A novel immunosensor for rapid separation-free determination of carcinoembryonic antigen (CEA) in human serum is proposed. The immunosensor is prepared by co-immobilizing thionine and horseradish peroxidase (HRP)-labeled CEA antibody on a glassy carbon electrode (GCE) through covalently binding them to GCE with a glutaraldehyde (GA) linkage. The electrochemical behavior of the immobilized thionine displays a surface-controlled electrode process with an average electron transfer rate constant of 4.74+/-2.99 s(-1). It can be used as an electron transfer mediator for enzymatic activity detection of the HRP-labeled antibody to CEA. After the immunosensor is incubated with CEA solution at 23 degrees C for 40 min, the access of activity center of the HRP to thionine is partly inhibited, which leads to a linear decrease in the catalytic efficiency of the HRP to the oxidation of immobilized thionine by H(2)O(2) at -300 mV over two CEA concentration ranges from 0.5 to 3.0 and 3.0 to 167 ng/ml. Under optimal conditions, the detection limit for the CEA immunoassay is 0.1 ng/ml at three times background noise. The immunosensor shows good accuracy and acceptable storage stability, precision and reproducibility with intra-assay CVs of 6.1% and 5.8% at 2.5 and 50 ng/ml CEA, respectively, and an inter-assay CV of 6.3% at 50 ng/ml. This method is economical and shortens the analytical time, making it potentially attractive for clinical immunoassays.

摘要

提出了一种用于快速无分离测定人血清中癌胚抗原(CEA)的新型免疫传感器。该免疫传感器是通过将硫堇和辣根过氧化物酶(HRP)标记的CEA抗体通过戊二醛(GA)键共价结合到玻碳电极(GCE)上共固定制备而成。固定化硫堇的电化学行为显示出表面控制的电极过程,平均电子转移速率常数为4.74±2.99 s(-1)。它可用作电子转移介质,用于检测HRP标记的CEA抗体的酶活性。免疫传感器在23℃下与CEA溶液孵育40分钟后,HRP的活性中心与硫堇的接触部分受到抑制,这导致在-300 mV下,HRP对H(2)O(2)氧化固定化硫堇的催化效率在两个CEA浓度范围(0.5至3.0和3.0至167 ng/ml)内呈线性下降。在最佳条件下,CEA免疫测定的检测限在三倍背景噪声下为0.1 ng/ml。该免疫传感器具有良好的准确性和可接受的储存稳定性、精密度和重现性,在2.5和50 ng/ml CEA时的批内变异系数分别为6.1%和5.8%,在50 ng/ml时的批间变异系数为6.3%。该方法经济且缩短了分析时间,使其在临床免疫测定中具有潜在吸引力。

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