首页> 外文期刊>Analytical Chemistry >HYDROGEN PEROXIDE SENSOR BASED ON COIMMOBILIZED METHYLENE GREEN AND HORSERADISH PEROXIDASE IN THE SAME MONTMORILLONITE-MODIFIED BOVINE SERUM ALBUMIN-GLUTARALDEHYDE MATRIX ON A GLASSY CARBON ELECTRODE SURFACE
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HYDROGEN PEROXIDE SENSOR BASED ON COIMMOBILIZED METHYLENE GREEN AND HORSERADISH PEROXIDASE IN THE SAME MONTMORILLONITE-MODIFIED BOVINE SERUM ALBUMIN-GLUTARALDEHYDE MATRIX ON A GLASSY CARBON ELECTRODE SURFACE

机译:基于共修饰的亚甲基绿和辣根过氧化物酶的过氧化氢传感器在相同的蒙脱土修饰的牛血清白蛋白-谷丙醛基质中的碳-碳电极表面

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摘要

A new approach to construct a second-generation amperometric biosensor is described. The classical dye methylene green as a probing-needle mediator and horseradish peroxidase as a base enzyme were coimmobilized in the same montmorillonite-modified bovine serum albumin (BSA)-glutaraldehyde matrix to construct a H2O2 sensor. The immobilization matrix was formed from the pretreated sodium montmorillonite colloid in which the enzyme and the cross-linker were dissolved. Immobilization of methylene green from the dye mother solution was attributed to the adsorption function of the montmorillonite, whereas immobilization of horseradish peroxidase was attributed to the cross-linking function of the BSA-glutaraldehyde as usual. Cyclic voltammetry and potentiostatic measurements indicated that methylene green efficiently mediated electrons from the base electrode to the enzyme in the matrix. The sensor responded rapidly to low H2O2 concentration and achieved 95% of the steady-state current in less than 20 s, with a detection limit of 4.0 x 10(-7) M H2O2.
机译:描述了一种构造第二代安培生物传感器的新方法。在相同的蒙脱土修饰的牛血清白蛋白(BSA)-戊二醛基质中,将经典的染料亚甲基绿作为探针的介体,辣根过氧化物酶作为基础酶,共固定在一个H2O2传感器上。由预处理的蒙脱土钠胶体形成固定化基质,其中溶解了酶和交联剂。通常,染料母液中亚甲基绿的固定归因于蒙脱石的吸附功能,而辣根过氧化物酶的固定归因于BSA-戊二醛的交联功能。循环伏安法和恒电位测量表明,亚甲基绿有效地介导了从基极到基质中酶的电子。传感器对低H2O2浓度迅速做出响应,并在不到20 s的时间内达到了稳态电流的95%,检测极限为4.0 x 10(-7)M H2O2。

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