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经构象变构调节固定在氧化还原聚合物内的对羟基苯乙酸羟化酶还原酶组件对还原型 β-烟酰胺腺嘌呤二核苷酸进行调谐的安培检测。

Tuned Amperometric Detection of Reduced β-Nicotinamide Adenine Dinucleotide by Allosteric Modulation of the Reductase Component of the p-Hydroxyphenylacetate Hydroxylase Immobilized within a Redox Polymer.

机构信息

School of Chemistry, Institute of Science, Biochemistry-Electrochemistry Research Unit (BECRU) , Suranaree University of Technology , 30000 Nakhon Ratchasima , Thailand.

Analytical Chemistry, Center for Electrochemical Sciences (CES) , Ruhr-University Bochum , 44780 Bochum , Germany.

出版信息

Anal Chem. 2018 May 1;90(9):5703-5711. doi: 10.1021/acs.analchem.7b05467. Epub 2018 Apr 16.

DOI:10.1021/acs.analchem.7b05467
PMID:29633834
Abstract

We report the fabrication of an amperometric NADH biosensor system that employs an allosterically modulated bacterial reductase in an adapted osmium(III)-complex-modified redox polymer film for analyte quantification. Chains of complexed Os(III) centers along matrix polymer strings make electrical connection between the immobilized redox protein and a graphite electrode disc, transducing enzymatic oxidation of NADH into a biosensor current. Sustainable anodic signaling required (1) a redox polymer with a formal potential that matched the redox switch of the embedded reductase and avoided interfering redox interactions and (2) formation of a cross-linked enzyme/polymer film for stable biocatalyst entrapment. The activity of the chosen reductase is enhanced upon binding of an effector, i.e. p-hydroxy-phenylacetic acid ( p-HPA), allowing the acceleration of the substrate conversion rate on the sensor surface by in situ addition or preincubation with p-HPA. Acceleration of NADH oxidation amplified the response of the biosensor, with a 1.5-fold increase in the sensitivity of analyte detection, compared to operation without the allosteric modulator. Repetitive quantitative testing of solutions of known NADH concentration verified the performance in terms of reliability and analyte recovery. We herewith established the use of allosteric enzyme modulation and redox polymer-based enzyme electrode wiring for substrate biosensing, a concept that may be applicable to other allosteric enzymes.

摘要

我们报告了一种安培 NADH 生物传感器系统的制造,该系统在适应的锇(III)- 配合物修饰的氧化还原聚合物膜中使用变构调节的细菌还原酶,用于分析物定量。沿基质聚合物链的配位 Os(III)中心链在固定化氧化还原蛋白和石墨电极盘之间建立电连接,将 NADH 的酶促氧化转化为生物传感器电流。可持续的阳极信号需要(1)具有与嵌入还原酶的氧化还原开关匹配的形式电势的氧化还原聚合物,以避免干扰的氧化还原相互作用,以及(2)形成交联酶/聚合物膜以稳定固定化生物催化剂。选择的还原酶的活性在结合效应物(即对羟基苯乙酸(p-HPA))时增强,允许通过原位添加或与 p-HPA 预孵育在传感器表面上加速底物转化率。NADH 氧化的加速放大了生物传感器的响应,与没有变构调节剂的操作相比,分析物检测的灵敏度提高了 1.5 倍。对已知 NADH 浓度的溶液进行重复定量测试验证了该方法在可靠性和分析物回收率方面的性能。我们在此建立了变构酶调节和基于氧化还原聚合物的酶电极布线用于底物生物传感的用途,这一概念可能适用于其他变构酶。

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