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一种用于测定甲酸盐的安培型双酶传感器,采用辅因子再生技术。

An amperometric bi-enzyme sensor for determination of formate using cofactor regeneration.

作者信息

Mak Karen K W, Wollenberger Ulla, Scheller Frieder W, Renneberg Reinhard

机构信息

Sino-German Nano-Analytical Lab (SiGNAL) and Department of Chemistry, The Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, Hong Kong.

出版信息

Biosens Bioelectron. 2003 Aug 15;18(9):1095-100. doi: 10.1016/s0956-5663(02)00245-2.

Abstract

A biosensor for detection of formate at submicromolar concentrations has been developed by co-immobilizing formate dehydrogenase (FDH, E.C. 1.2.1.2), salicylate hydroxylase (SHL, E.C. 1.14.13.1) and NAD(+) linked to polyethylene glycol (PEG-NAD(+)) in a poly(vinyl alcohol) (PVA) matrix in front of a Clark-electrode. The principle of the bi-enzyme scheme is as follows: formate dehydrogenase converts formate into carbon dioxide using PEG-NAD(+). Corresponding PEG-NADH produced is then oxidized to PEG-NAD(+) by salicylate hydroxylase using sodium salicylate and oxygen. The oxygen consumption is monitored with the Clark-electrode. The advantages of this biosensor approach are the effective re-oxidation of PEG-NADH, and the entrapment of PEG-NAD(+) resulting in avoiding the addition of expensive cofactor to the working medium for each measurement. This bi-enzyme sensor has achieved a linear range of 1-300 microM and a detection limit of 1.98 x 10(-7) M for formate (S/N=3), with the response time of 4 min. The working stability is limited to 7 days due to the inactivation of the enzymes. Only sodium salicylate was needed in milli-molar amounts.

摘要

通过在Clark电极前的聚乙烯醇(PVA)基质中共固定甲酸脱氢酶(FDH,E.C. 1.2.1.2)、水杨酸羟化酶(SHL,E.C. 1.14.13.1)和与聚乙二醇连接的NAD⁺(PEG-NAD⁺),开发了一种用于检测亚微摩尔浓度甲酸的生物传感器。双酶体系的原理如下:甲酸脱氢酶利用PEG-NAD⁺将甲酸转化为二氧化碳。然后,产生的相应PEG-NADH被水杨酸羟化酶利用水杨酸钠和氧气氧化为PEG-NAD⁺。用Clark电极监测氧气消耗。这种生物传感器方法的优点是PEG-NADH的有效再氧化,以及PEG-NAD⁺的截留,从而避免了每次测量时向工作介质中添加昂贵的辅因子。这种双酶传感器对甲酸的线性范围为1-300 μM,检测限为1.98×10⁻⁷ M(S/N = 3),响应时间为4分钟。由于酶的失活,工作稳定性限制为7天。仅需要毫摩尔量的水杨酸钠。

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