A glucose biosensor using methyl viologen redox mediator on carbon film electrodes

A new methyl viologen-mediated amperometric enzyme electrode sensitive to glucose has been developed using carbon film electrode substrates. Carbon film electrodes from resistors fabricated by pyrolytic deposition of carbon were modified by immobilization of glucose oxidase through cross-linking with glutaraldehyde in the presence of bovine serum albumin. The mediator, methyl viologen, was directly immobilised with the enzyme together with Nafion cation-exchange polymer. The electrochemistry of the glucose oxidase/methyl viologen modified electrode was investigated by cyclic voltammetry and by electrochemical impedance spectroscopy. The biosensor response to glucose was evaluated amperometrically; the detection limit was 20 μM, the linear range extended to 1.2 mM and the reproducibility of around 3%. When stored in phosphate buffer at 4 °C and used every day, the sensor showed good stability over more several weeks.     

The electrochemical behaviour of ferrocene in a photocurable poly(methyl methacrylate-co-2-hydroxylethyl methacrylate) film for a glucose biosensor

A single-step fabrication of a glucose biosensor with simultaneous immobilization of both ferrocene mediator and glucose oxidase in a photocurable methacrylic film consisting of poly(methyl methacrylate-co-2-hydroxylethyl methacrylate) was reported. The entrapped ferrocene showed reversible redox behaviour in the photocured film and no significant leaching of both entrapped ferrocene and enzyme glucose oxidase was observed because of the low water absorption properties of the co-polymer films. From electrochemical studies, ferrocene entrapped in the co-polymer film demonstrated slow diffusion properties. A linear glucose response range of 2-11 mM was obtained at low applied potential of +0.25 V. The glucose biosensor fabricated by this photocuring method yielded sensor reproducibility and repeatability with relative standard deviation of <10% and long-term stability of up to 14 days. The main advantage of the use of photocurable procedure is that biosensor membrane fabrication can be performed in a single step without any lengthy chemical immobilization of enzyme.     

A novel nanocomposite matrix based on graphene oxide and ferrocene-branched organically modified sol–gel/chitosan for biosensor application

A novel platform for the fabrication of a glucose biosensor was successfully constructed by entrapping glucose oxidase (GOD) in a ferrocene (Fc)-branched organically modified silica material (ormosil)/chitosan (CS)/graphene oxide (GO) nanocomposite. The morphology, structure, and electrochemistry of the nanocomposite were characterized by transmission electron microscopy, X-ray powder diffraction, UV–vis spectroscopy, Fourier transform infrared spectroscopy, and electrochemical techniques. Results demonstrated that the proposed electrochemical platform not only provided an excellent microenvironment to maintain the bioactivity of the immobilized enzyme, but also effectively prevented the leakage of both the enzyme and mediator from the matrix and retained the electrochemical activity of Fc. Furthermore, dispersing GO within the Fc-branched ormosil/CS matrix could significantly improve the stability of GO and make it exhibit a positive charge, which was more favorable for the further immobilization of biomolecules, such as GOD, with higher loading. Moreover, it could also improve the conductivity of the matrix film and facilitate the electron shuttle between the mediator and electrode. Under optimal conditions, the designed biosensor to glucose exhibited a wide and useful linear range of 0.02 to 5.39 mM with a low detection limit of 6.5 μM. The value of K _M ^app was 4.21 mM, indicating that the biosensor possesses higher biological affinity to glucose. The present approach could be used efficiently for the linkage of other redox mediators and immobilize other biomolecules in the process of fabricating novel biosensors.     

Optimized preparation and scanning electrochemical microscopy analysis in feedback mode of glucose oxidase layers grafted onto conducting carbon surfaces

An optimized immobilization procedure based on the electroreduction of aryldiazonium salt followed by covalent attachment of a cross-linked hydrogel was used to graft glucose oxidase on a carbon surface. Scanning electrochemical microscopy (SECM) and cyclic voltammetry were used to follow the construction steps of the modified electrode. By adjusting the compactness of the layer through the electrografting reaction, the penetration of the mediator through the layer can be controlled to allow the monitoring of the enzymatic activity by both cyclic voltammetry and SECM in feedback mode. The enzymatic activity of the film is finally characterized by SECM.     

基于仿生聚多巴胺膜和纳米金的酶固定化平台的构建

首次以仿生聚多巴胺膜为功能基底膜并结合使用纳米金, 构建了一种高导电性、稳健的酶生物分子固定化平台. 以固定辣根过氧化物酶(HRP)为例, 发展了一种新的电化学酶传感器用于H2O2的测定. 结果表明, 酶传感器借助聚多巴胺膜对基底电极的高结合力及其高生物亲和性与电活性, 并协同纳米金的“电子通道”作用, 不仅可以实现酶分子在电极表面的大量而高活性的固定化, 而且能促进电子在酶活性中心和电极表面间的快速传递. 与采用其它常见聚合物材料(例如壳聚糖)的酶传感器比较, 以聚多巴胺/纳米金固定化平台发展的酶传感器具有更优良的检测H2O2的性能. 其对H2O2的检测线性范围为4.0×10－7～4.5×10－4 mol•L－1, 检测限为3.7×10－7 mol•L－1, 灵敏度为100.2 μA•L•mmol－1. 此外, 该酶传感器还具有优良的检测重现性和存贮稳定性, 以及较好的抗干扰能力.     

Amperometric glucose-responding property of enzyme electrodes fabricated by covalent immobilization of glucose oxidase on conducting polymer films with macroporous structure

Macroporous conducting polymer films were prepared by the electrochemical copolymerization of 3-methylthiophene and thiophene-3-acetic acid on the ITO-coated glass plates bearing different sizes of polystyrene template particles, and enzyme electrodes were fabricated by covalent immobilization of glucose oxidase on the macroporous copolymer films. It was found that the doping level and conductivity of the copolymer films was significantly affected by the treatment with solvent to remove the polystyrene particles, which was considered to result in deterioration in amperometric glucose-responding property of the enzyme electrodes fabricated with the copolymer films. Three-dimensionally ordered macroporous structure on the copolymer films led to enhancement of amperometric response of the enzyme electrodes, and this effect was attributed to the geometry of the interconnected channel structure formed by the linkage of macropores. It was suggested that the amperometric response of the enzyme electrodes was determined by whether the interconnected channel structure on the copolymer films had long distance regularity and a proper size to allow the enzyme and electron-mediator molecules to penetrate into the interior pores of the copolymer film. In particular, the interconnected channel structure seemed to play an important role in the electron-transfer reaction between the mediator molecules and the surface of electrodes.     

Glucose Microbiosensor Based on MnO2 and Glucose Oxidase Modified Carbon Fiber Microelectrode

A glucose microbiosensor has been developed using electrochemical codeposition of glucose oxidase (GOx) along with MnO₂ as mediator, onto a single carbon fiber microelectrode. A two‐step deposition of only MnO₂ initially and then of MnO₂ in the presence of GOx has been introduced to ensure appropriate activity of the mediator. Several parameters such as deposition potential and time, concentration levels etc. have been characterized and optimized. A thin Nafion film was applied as an immobilization/encapsulation and interference‐free protective layer. The proposed microbiosensor was employed as an amperometric glucose detector at pH 7.5 at an operating potential of +0.58 V (vs. Ag/AgCl). The microbiosensor is characterized by a well‐reproducible amperometric response, linear signal‐to‐glucose concentration range from 1.5 mmol L^?1 to 15 mmol L^?1, and a limit of detection (S/N=3) of 0.8 mmol L^?1. The microbiosensor exhibits good stability over more than ten hours of continuous measurement.     

电化学酶传感器在环境污染监测中的应用

电化学酶传感器是一种应用广泛的生物传感器,它将酶及其底物相互作用的特异性与电化学的强大分析功能相结合,已经被广泛应用于药理学、临床、食品、农业以及环境监测中。制备电化学酶传感器的关键步骤是酶的固定化,选择用于制备电化学酶传感器的合适的酶固定化方法,在传感器电子转移动力学、稳定性和重现性等方面起着主要作用。本文在阐述电化学酶传感器工作原理的基础上,简要介绍了用于电化学酶传感器制备过程中的酶固定化方法,重点讨论了电化学酶传感器在监测环境中广泛存在的有机污染物、无机污染物和重金属等方面的应用,并对电化学酶传感器的发展方向进行了展望。     

Direct electrochemistry of cytochrome c immobilized on a novel macroporous gold film coated with a self-assembled 11-mercaptoundecanoic acid monolayer

We have successfully constructed a novel gold film with open interconnected macroporous walls of nanoparticles by combining the hydrogen bubble dynamic template synthesis with galvanic replacement reaction. After modified by a self-assembled monolayer (SAM) of 11-mercaptoundecanoic acid (MUA), the three-dimensionally (3D) interconnected macroporous Au film has been used as a biocompatible substrate for the immobilization of cytochrome c. The morphology, structure and electrochemical features of the modified and unmodified macroporous Au films were characterized by field-emission scanning electron microscopy (FESEM), energy-dispersive X-ray (EDX), cyclic voltammetry (CV) and electrochemical impedance spectroscopy (EIS). The results reveal that the resultant films had a large electroactive surface area for high protein loading, enhanced electron transfer of cytochrome c, retained electrochemical activity, good stability and repeatability. And the excellent electrochemical behaviors could be attributed to the hierarchical structure of the macroporous Au film constructed by nanoparticles.     

Glucose and lactate biosensors prepared by a layer-by-layer deposition of concanavalin A and mannose-labeled enzymes: electrochemical response in the presence of electron mediators.

An electrochemical response of glucose and lactate biosensors which were prepared by coating a platinum electrode with a thin film composed of concanavalin A and mannose-labeled glucose oxidase (GOx) or lactate oxidase (LOx) was evaluated in the presence of ferrocene derivatives as electron mediator. Both glucose and lactate biosensors showed catalytic current to glucose and lactate, respectively, in cyclic voltammetry, suggesting that the ferrocene derivatives can mediate electron transport smoothly from the reduced forms of GOx and LOx in the thin films to the electrode. Among the three kinds of ferrocene derivatives used, ferrocenylmethanol was found to be the most suitable electron mediator because of its low oxidation potential. The glucose and lactate sensors gave useful calibration graphs, in which higher detection limits were reached as compared with those observed when the sensors were operated in the absence of electron mediator.     

A control over accessibility of immobilized enzymes through porous coating layer

We report immobilization of an enzyme by layer-by-layer (LbL) film deposition technique. All the enzyme layers, including the inner ones, contributed to the activity. We put-forwarded additional coating layers to protect the enzymes. To control the accessibility of the enzymes beneath the coating layer, pores have been introduced. Our results show controlled accessibility of immobilized enzymes in solid-state matrices.     

Guanine/Ionic Liquid Derived Ordered Mesoporous Carbon Decorated with AuNPs as Efficient NADH Biosensor and Suitable Platform for Enzymes Immobilization and Biofuel Cell Design

Guanine‐ionic liquid derived ordered mesoporous carbon (GIOMC) decorated with gold nanoparticles was used as electrocatalyste for NADH oxidation and electrochemical platform for immobilization of glucose dehydrogenase (GDH) enzyme. The resulting GIOMC/AuNPs on the glassy carbon electrode can be used as novel redox‐mediator free for NADH sensing and this integrated system (GIOMC/AuNPs/GDH) shows excellent electrocatalytic activity toward glucose oxidation. Furthermore, the ionic liquid derived ordered mesoporous carbon derivate with Ph‐SO₃H (IOMC‐PhSO₃H) decorated with AuNPs has been developed to bilirubin oxidase enzyme (BOD) immobilization and the GC/IOMC‐PhSO₃H/BOD integrated system shows excellent bioelectrocatalytic activity toward oxygen reduction reaction. The proposed mesostructured platforms decorated by AuNPs have been developed to enhance mass transfer and charge transfer from biocatalyst to electrode, leading these bioanode and biocathode used for biofuel cell assembly. Integration designed bioanode and biocathode yielding a membrane‐less glucose/O₂ biofuel cell with power density of 33 (mW.cm⁻²) at 257 mV. The open circuit voltage of this biofuel cell and maximum produced current density were 508 mV and 0.252 (mA.cm⁻²) respectively.     

Electrochemical Oxidation of Glucose Using Mutant Glucose Oxidase from Directed Protein Evolution for Biosensor and Biofuel Cell Applications

In this study, electrochemical characterisation of glucose oxidation has been carried out in solution and using enzyme polymer electrodes prepared by mutant glucose oxidase (B11-GOx) obtained from directed protein evolution and wild-type enzymes. Higher glucose oxidation currents were obtained from B11-GOx both in solution and polymer electrodes compared to wt-GOx. This demonstrates an improved electrocatalytic activity towards electrochemical oxidation of glucose from the mutant enzyme. The enzyme electrode with B11-GOx also showed a faster electron transfer indicating a better electronic interaction with the polymer mediator. These encouraging results have shown a promising application of enzymes developed by directed evolution tailored for the applications of biosensors and biofuel cells.     

生物功能电极 III. 葡萄糖氧化酶的电化学固定化研究

利用磷酸盐缓冲溶液中吡咯的电聚合, 将葡萄糖氧化酶(GOD)包埋在聚吡咯(PPy)基质中以构成生物功能电极。讨论了溶液pH和聚合电位对酶固定化的影响, 并用IR和交流阻抗谱对酶膜进行表征。GOD的固定化只有当pH>5.5时才能实现, 由此推测酶是以带负电的粒子嵌入PPy的。交流阻抗谱表明这一电极具有有界多孔电极的特征。探索了酶与电子传递体Fe(CN)_6~(3-)同时固定化的可行性。电化学固定化的GOD保持其生物催化活性, 酶反应表观上遵循Michealis-Menten动力学。     

生物功能电极 Ⅲ.葡萄糖氧化酶的电化学固定化研究

利用磷酸盐缓冲溶液中吡咯的电聚合,将葡萄糖氧化酶(GOD)包埋在聚吡咯(PPy)基质中以构成生物功能电极。讨论了溶液pH和聚合电位对酶固定化的影响,并用IR和交流阻抗谱对酶膜进行表征。GOD的固定化只有当pH>5.5时才能实现,由此推测酶是以带负电的粒子嵌入PPy的。交流阻抗谱表明这一电极具有有界多孔电极的特征。探索了酶与电子传递体Fe(CN)_6~(3-)同时固定化的可行性。电化学固定化的GOD保持其生物催化活性,酶反应表观上遵循Michealis-Menten动力学。     

Amine-terminated organosilica nanosphere functionalized prussian blue for the electrochemical detection of glucose

A new glucose biosensor had been developed by immobilizing positively charged gold nanoparticles (PGNs) on organosilica nanosphere functionalized prussian blue (OSiFPB)-modified gold electrode. The OSiFPB compound could not only effectively prevent the leakage of the PB mediator during measurements, but also easily form stable film on the electrode surface with efficient redox-activity and excellent conductivity. Furthermore, with the negatively charged surface of OSiFPB, this film could be used as an interface to adsorb the PGNs, which provided a congenial microenvironment for adsorbing biomolecules and decreased the electron-transfer impedance. So, with glucose oxidase as a model biomolecular, the proposed sensor showed rapid and highly sensitive amperometric response to glucose and this immobilization approach effectively improved the stability of the electron-transfer mediator. This work would be promising for construction of biosensor and bioelectronic devices.     

Effect of substrate inhibition and cooperativity on the electrochemical responses of glucose dehydrogenase. Kinetic characterization of wild and mutant types

Thanks to its insensitivity to dioxygen and to its good catalytic reactivity, and in spite of its poor substrate selectivity, quinoprotein glucose dehydrogenase (PQQ-GDH) plays a prominent role among the redox enzymes that can be used for analytical purposes, such as glucose detection, enzyme-based bioaffinity assays, and the design of biofuel cells. A detailed kinetic analysis of the electrochemical catalytic responses, leading to an unambiguous characterization of each individual steps, seems a priori intractable in view of the interference, on top of the usual ping-pong mechanism, of substrate inhibition and of cooperativity effects between the two identical subunits of the enzyme. Based on simplifications suggested by extended knowledge previously acquired by standard homogeneous kinetics, it is shown that analysis of the catalytic responses obtained by means of electrochemical nondestructive techniques, such as cyclic voltammetry, with ferrocene methanol as a mediator, does allow a full characterization of all individual steps of the catalytic reaction, including substrate inhibition and cooperativity and, thus, allows to decipher the reason that makes the enzyme more efficient when the neighboring subunit is filled with a glucose molecule. As a first practical illustration of this electrochemical approach, comparison of the native enzyme responses with those of a mutant (in which the asparagine amino acid in position 428 has been replaced by a cysteine residue) allowed identification of the elementary steps that makes the mutant type more efficient than the wild type when cooperativity between the two subunits takes place, which is observed at large mediator and substrate concentrations. A route is thus opened to structure-reactivity relationships and therefore to mutagenesis strategies aiming at better performances in terms of catalytic responses and/or substrate selectivity.     

Polymer-Complex Mediated Enzyme Electrodes for Amperometric Determination of Glucose

The immobilized enzyme chemically modified solid-state electrodes based on bilayer-film coating for amperometric determination of glucose have been fabricated and their sensor characteristics have been examined. The electrode substrate was coated with two kinds of polymeric films in a bilayer state, that is, System I: first with the cobalt tetrakis(o-aminophenyl)porphyrin polymer (poly-CoTAPP) film and then with an enzyme film consisting of bovine serum albumin and glucose oxidase (GOx), and System II: first with the Ru(NH₃)³⁺ ₆-containing montmorillonite clay film and then with the GOx enzyme film. The glucose concentration could be monitored by measuring the currents corresponding to the O₂ reduction and the H₂O₂ reduction which are electrocatalyzed by the poly-CoTAPP film (System I) and the clay film (System II), respectively. The reproducible relationship between glucose concentration and sensor output was obtained for both systems with a dynamic range of ～ 1-100 mM (for System I as an electrochemical detector for a flow injection analysis) and ～0.4-4 mM (for System II). In addition, the sensors showed long-term stability (more than 1 and 2 months in System I and System II, respectively) and relatively rapid response (response times of System I and System II are ? 5-10 and 40-60 s, respectively).     

Development of Biosensors Based on Immobilization of Enzymes in Eastman AQ Polymer Coated with a Layer of Nafion

Abstract

A fast and simple procedure to prepare enzyme electrode is presented herein. A blend of amorphous polyester cationic exchangers (AQ 29D:AQ 55D; ratio 1:1) dispersed in water has been used for the immobilization of l-amino acid, choline, galactose or glucose oxidase enzymes at the surface of a platinum electrode. The resulting polymer-enzyme film was covered by a thin layer of Nafion to avoid its subsequent dissolution in water. The assays are based on the electrochemical detection of enzymatically generated hydrogen peroxide. Good amperometric responses were obtained with each of these enzyme electrodes. The major advantage in using this water dispersed polymer lies in its ability to dissolve the enzyme without any significative loss of enzymatic activity.     

Electrochemical Reduction of a Conjugated Cinnamic Acid Diazonium Salt as an Immobilization Matrix for Glucose Biosensor

Initial results on the synthesis of a new conjugated diazonium salt of trans‐4‐cinnamic acid diazonium fluoroborate, which is used for the chemical modification of the glassy carbon (GC) electrode with trans‐4‐cinnamic acid groups through electrochemical reduction, and direct covalent immobilization of glucose oxidase (GOD) on the cinnamic acid groups are presented. The chemically modified GC electrode exhibits a good selectivity relative to the bare GC electrode for the various possible interfering compounds in glucose analysis: namely ascorbic acid and 4‐acetamidophenol. Covalent immobilization of GOD on the chemically modified GC electrode produces a biosensor which responds to glucose concentration changes in the presence of a soluble redox mediator (ferrocenemethanol). The chemical modification of GC by cinnamic acid groups is potentially useful for the attachment of other enzymes and biochemical reagents.