Coupled triple phase boundary processes: Liquid–liquid generator–collector electrodes

Electrochemical processes at liquid–liquid–electrode interfaces involve simultaneous ion transfer and electron transfer. When driven at triple phase boundary electrode systems, electron and ion transfer occur in the same interfacial reaction zone. In this report, preliminary work with a novel electrode system based on two coupled triple phase boundary reaction zones is described. An interdigitated gold band array with 7 μm gold bands separated by 13 μm gaps is employed immersed in aqueous electrolyte with a water-immiscible solution of the redox system N,N-diethyl-N′N′-didodecyl-phenylenediamine (DDPD) in 4-(3-phenylpropyl)-pyridine (PPP) immobilized on the surface. Well-defined generator–collector feedback currents are observed which depend on the volume of deposit, the concentration of the redox system, and the nature of the aqueous electrolyte.     

Immobilization and electrochemical behavior of gold nanoparticles modified leukemia K562 cells and application in drug sensitivity test

A new strategy for immobilization of tumor cells on electrode surface and accelerating electron transfer between electrode and the immobilized cells was proposed to study the electrochemical behavior of cells and the effect of antitumor drug on cell viability. The leukemia K562 cells immobilized in a microporous cellulose membrane were firstly modified with colloidal gold nanoparticles to retain efficiently the activity of immobilized living tumor cells and promote electron transfer between electroactive centers of the cells and the electrode, exhibiting a well-defined anodic peak of guanine at +0.830 V at 50 mV s⁻¹. The electrochemical response could be used to describe cell growth and evaluate the effectiveness of antitumor drug methotrexate on tumor cells. The proposed method offered potential advantages for drug sensitivity test with little usage of cells. It could be developed as a convenient means for the study of the tumor cells growth and the cytotoxicity of antitumor drugs.     

Direct electrochemistry and electrocatalysis of hemoglobin entrapped in composite matrix based on chitosan and CaCO3 nanoparticles

The direct electron transfer between hemoglobin (Hb) and the underlying glassy carbon electrode (GCE) can be readily achieved via a high biocompatible composite system based on biopolymer chitosan (CHT) and inorganic CaCO₃ nanoparticles (nano-CaCO₃). Cyclic voltammetry of Hb-CHT/nano-CaCO₃/GCE showed a pair of stable and quasi-reversible peaks for HbFe(III)/Fe(II) redox couple in pH 7.0 buffer. The electrochemical reaction of Hb immobilized in CHT/nano-CaCO₃ composite matrix exhibited a surface-controlled process accompanied by electron and proton transfer. The electron transfer rate constant was estimated to be 1.8 s⁻¹. This modified electrode showed a high thermal stability up to 60 °C. The apparent Michaelis–Menten constant was calculated to be 7.5 × 10⁻⁴ M, indicating a high catalytic activity of the immobilized Hb toward H₂O₂. The interaction between Hb and this nano-hybrid material was also investigated using FT-IR and UV–vis spectroscopy, indicating that Hb retained its native structure in this hybrid matrix.     

High performance bioanode based on direct electron transfer of fructose dehydrogenase at gold nanoparticle-modified electrodes

The direct electron transfer reaction of fructose dehydrogenase (FDH) from Gluconobacter sp. on alkanethiol-modified gold nanoparticles (AuNPs) was examined. AuNP-modified electrodes were simply fabricated by depositing citrate-reduced gold nanoparticles onto a gold electrode and carbon fiber paper and then covering the surface with a self-assembled monolayer of alkanethiols. The immobilization of AuNPs provided a large effective surface area for the adsorption of FDH. Catalytic oxidation currents based on the direct electron transfer reaction of FDH were observed from a potential about ?100 mV (vs. Ag/AgCl, 3 M NaCl) in the presence of d-fructose without a mediator. The current density reached as high as 14.3 ± 0.93 mA/cm² (at +500 mV), which was achieved in the presence of 200 mM d-fructose by immobilization of FDH on 2-mercaptoethanol-modified AuNP/carbon fiber paper electrodes.     

Surface poisoning during electrocatalytic monosaccharide oxidation reactions at gold electrodes in alkaline medium

In the present study, the surface poisoning of electrocatalytic monosaccharide oxidation reactions at gold electrodes were investigated. In the cyclic voltammetric studies, the electrocatalytic oxidation of aldohexose and aldopentose type monosaccharides, aminosugars, acetyl-glucosamine and glucronamide were observed at gold plate electrodes in alkaline medium. However, in controlled-potential electrolytic studies ranging −0.3 to −0.2 V in reaction solutions, current flows during electrolyses decreased quickly with time, except when glucosamine was used as a substrate.Results from surface enhanced infrared adsorption (SEIRA) spectroscopic measurements at an evaporated gold electrode for the electrocatalytic oxidation of glucose in 0.1 mol dm⁻³ NaOH at −0.3 V and Gaussian simulated spectra indicated that the gluconic acid as a 2-electron oxidation product and/or its analogs adsorbed onto the gold surface. Electrochemical quartz crystal microbalance (EQCM) measurement results, along with surface adsorption results from surface poisoning at the gold electrode during electrolytic reactions, suggested that gluconic acid and/or its analogs adsorbed vertically onto electrode surfaces in a full monolayer packing-like conformation. In the case of the electro oxidation of glucosamine in 0.1 mol dm⁻³ NaOH at −0.2 V, the obtained SEIRA spectra and EQCM results, clearly indicated that the glucosaminic acid as a 2-oxidation glucosamine product did not strongly bind onto the gold electrode surface.     

Direct electron transfer of cytochrome c and its biosensor based on gold nanoparticles/room temperature ionic liquid/carbon nanotubes composite film

A robust and effective composite film based on gold nanoparticles (GNPs)/room temperature ionic liquid (RTIL)/multi-wall carbon nanotubes (MWNTs) modified glassy carbon (GC) electrode was prepared by a layer-by-layer self-assembly technique. Cytochrome c (Cyt c) was successfully immobilized on the RTIL-nanohybrid film modified GC electrode by electrostatic adsorption. Direct electrochemistry and electrocatalysis of Cyt c were investigated. The results suggested that Cyt c could be tightly adsorbed on the modified electrode. A pair of well-defined quasi-reversible redox peaks of Cyt c was obtained in 0.10 M, pH 7.0 phosphate buffer solution (PBS). RTIL-nanohybrid film showed an obvious promotion for the direct electron transfer between Cyt c and the underlying electrode. The immobilized Cyt c exhibited an excellent electrocatalytic activity towards the reduction of H₂O₂. The catalysis currents increased linearly to the H₂O₂ concentration in a wide range of 5.0 × 10⁻⁵– 1.15 × 10⁻³ M. Based on the multilayer film, the third-generation biosensor could be constructed for the determination of H₂O₂.     

A molecular wire modified glassy carbon electrode for achieving direct electron transfer to native glucose oxidase

Here we describe a strategy for achieving direct electron transfer to native glucose oxidase (GOx), an enzyme in which the redox active centre is buried deep within the glycoprotein. To achieve this a glassy carbon electrode is modified with a mixed monolayer of 4-carboxyphenyl and a 20 Å long oligo(phenylethynyl) molecular wire (MW), assembled from the respective aryl diazonium salts. Subsequently GOx is adsorbed to the interface, followed by covalent attachment. The redox chemistry of the active centre of glucose oxidase, flavin adenine dinucleotide, was observed at an E_1/2 of –443 mV (vs. Ag|AgCl). The enzyme was shown to retain its activity. Most importantly, in the absence of oxygen the electrode was still able to biocatalytically turn over glucose at −400 mV, thereby demonstrating that the enzyme was being recycled back to its catalytically active oxidized form from its inactive reduced form. The rate of enzyme turnover was 1.1 s⁻¹.     

Synthesis,characterizations of silica-coated gold nanorods and its applications in electroanalysis of hemoglobin

Gold nanorods (GNRs) were synthesized by a seed–mediated growth approach followed by TEOS polymerization leading to the formation of silica layer surrounding the gold nanorod core. TEM images showed that the silica-coated gold nanorods (GNRs@SiO₂) were dispersed with an average aspect ratio of 3.1 for the GNRs cores and a uniform thickness of the silica shell. The core/shell nanocomposites were further used as efficient supports for the immobilization of hemoglobin (Hb) to fabricate a novel biosensor. The immobilized Hb showed an enhanced electron transfer for its heme Fe(III) to Fe(II) redox couple. This biosensor showed an excellent bioelectrocatalytic activity towards H₂O₂ with a linear range from 8.0 × 10⁻⁷ to 6.1 × 10⁻⁵ M, and the detection limit was 6.0 × 10⁻⁸ M at 3σ. The apparent Michaelis–Menten constant of the immobilized hemoglobin was calculated to be 0.13 mM.     

Mediated electron transfer with P450cin

P450cin stereoselectively hydroxylated its natural substrate 1,8-cineole to 2β-hydroxy-1,8-cineole in an electrochemical cell which allowed for substitution of the natural cofactor NADPH by artificial redox mediators. Cobalt sepulchrate, phenosafranine, safranine T, FAD and FMN enabled artificial electron transfer from the platinum electrode to P450cin via the redox partner protein cindoxin. The highest product formation, 6.50 ± 0.60 nmol (product) nmol (P450)^?1 min^?1 cm^?2, was achieved using cobalt sepulchrate. Surprisingly, phenosafranine and safranine T enabled electron transfer even in the absence of NADPH, cindoxin, and cindoxin reductase, thereby illustrating that none of the natural redox partners is needed for product formation.     

Enhanced electron transfer between gold nanoparticles and horseradish peroxidase reconstituted onto alkanethiol-modified hemin

Robust molecular bioelectronic devices require a programmable and efficient electronic communication between biological molecules and electrodes. With proteins it is often compromised by their uncontrollable assembly on electrodes that does not provide neither uniform nor efficient electron flow between proteins and electrodes. Here, horseradish peroxidase reconstituted onto C₁₁-alkanethiol-conjugated hemin and self-assembled onto the gold nanoparticle (NP)-modified electrodes via the exposed alkanethiol tail exhibits enhanced electron transfer (ET), proceeding via the gold NP relay with the ET rate constant approaching 115 s^− 1 vs. 14 s^− 1 shown on bare gold, by this offering an advanced controllable design of interfaces for bioelectronic devices based on heme-containing enzymes with a non-covalently bound heme.     

Amperometric glucose sensor based on glucose oxidase immobilized on gelatin-multiwalled carbon nanotube modified glassy carbon electrode

We investigated the direct electrochemistry of glucose oxidase (GOx) at gelatin-multiwalled carbon nanotube (GCNT) modified glassy carbon electrode (GCE). GOx was covalently immobilized onto GCNT modified GCE through the well known glutaraldehyde (GAD) chemistry. The immobilized GOx showed a pair of well-defined reversible redox peaks with a formal potential (E⁰′) of ? 0.40 V and a peak to peak separation (ΔE_p) of 47 mV. The surface coverage concentration (Г) of GOx in GCNT/GOx/GAD composite film modified GCE was 3.88 × 10^? 9 mol cm^? 2 which indicates the high enzyme loading. The electron transfer rate constant (k_s) of GOx immobilized onto GCNT was 1.08 s^? 1 which validates a rapid electron transfer processes. The composite film shows linear response towards 6.30 to 20.09 mM glucose. We observed a good sensitivity of 2.47 μA mM^?1 cm^? 2 for glucose at the composite film. The fabricated biosensor displayed two weeks stability. Moreover, it shows no response to 0.5 mM of ascorbic acid (AA), uric acid (UA), acetaminophen (AP), pyruvate (PA) and lactate (LA) which shows its potential application in the determination of glucose from human serum samples. The composite film exhibits excellent recovery for glucose in human serum at physiological pH with good practical applicability.     

Direct electrochemistry and electrocatalysis of hemoglobin in sodium alginate film on a BMIMPF6 modified carbon paste electrode

A room temperature ionic liquid (RTIL) modified carbon paste electrode was constructed based on the substitute of paraffin with 1-butyl-3-methyl-imidazolium hexafluorophosphate (BMIMPF₆) as binder for carbon paste. Direct electrochemistry and electrocatalytic behaviors of hemoglobin (Hb) entrapped in the sodium alginate (SA) hydrogel film on the surface of this carbon ionic liquid electrode (CILE) were investigated. The presence of IL in the CILE increased the electron transfer rate and provided a biocompatible interface. Hb remained its bioactivity on the surface of CILE and the SA/Hb modified electrode showed a pair of well-defined, quasi-reversible cyclic voltammetric peaks with the apparent standard potential (E^0′) at about −0.344 V (vs. SCE) in pH 7.0 Britton–Robinson (B–R) buffer solution, which was attributed to the Hb Fe(III)/Fe(II) redox couple. UV–Vis absorption spectra indicated that heme microenvironment of Hb in SA film was similar to its native status. Hb showed a thin-layer electrochemical behavior in the SA film with the direct electron transfer achieved on CILE without the help of electron mediator. Electrochemical investigation indicated that Hb took place one proton with one electron electrode process and the average surface coverage of Hb in the SA film was 3.2 × 10⁻¹⁰ mol/cm². The immobilized Hb showed excellent electrocatalytic responses to the reduction of H₂O₂ and nitrite.     

Design of a bioelectrocatalytic electrode interface for oxygen reduction in biofuel cells based on a specifically adapted Os-complex containing redox polymer with entrapped Trametes hirsuta laccase

The design of the coordination shell of an Os-complex and its integration within an electrodeposition polymer enables fast electron transfer between an electrode and a polymer entrapped high-potential laccase from the basidiomycete Trametes hirsuta. The redox potential of the Os^3+/2+-centre tethered to the polymer backbone (+ 720 mV vs. NHE) is perfectly matching the potential of the enzyme (+ 780 mV vs. NHE at pH 6.5). The laccase and the Os-complex modified anodic electrodeposition polymer were simultaneously precipitated on the surface of a glassy carbon electrode by means of a pH-shift to 2.5. The modified electrode was investigated with respect to biocatalytic O₂ reduction to H₂O. The proposed modified electrode has potential applications as biofuel cell cathode.     

Construction of an amperometric biosensor for xanthine via supramolecular associations

Xathine oxidase was chemically modified with β-cyclodextrin-branched carboxymethylcellulose and further supramolecularly immobilized on a gold electrode, previously coated with a monolayer of 1-adamantanyl residues. The electrode was employed for constructing an amperometric biosensor device, which showed linear response (poised at +700 mV vs. Ag/AgCl) toward xanthine concentration between 300 μM and 10.4 mM at pH 7.0. The biosensor reached 95% of steady-state current in about 14 s and its sensitivity was 8.2 mA/M cm². The enzyme electrode retained 93% of its initial activity after 3 weeks of storage at 4 °C in 50 mM sodium phosphate buffer, pH 7.0. The supramolecular nature of the immobilization approach was confirmed by cyclic voltammetry.     

Bioelectrocatalytic oxidation of glucose by hexose oxidase directly wired to graphite

Glucose-oxidizing enzymes are widely used in electrochemical biosensors and biofuel cells; in most applications glucose oxidase, an enzyme with non-covalently bound FAD and low capability of direct electronic communications with electrodes, is used. Here, we show that another glucose-oxidizing enzyme with a covalently bound FAD center, hexose oxidase (HOX), adsorbed on graphite, exhibits a pronounced non-catalytic voltammetric response from its FAD, at − 307 mV vs. Ag/AgCl, pH 7, characterized by the heterogeneous electron transfer (ET) rate constant of 29.2 ± 4.5 s^− 1. Direct bioelectrocatalytic oxidation of glucose by HOX proceeded, although, with a 350 mV overpotential relative to FAD signals, which may be connected with a limiting step in biocatalysis under conditions of the replacement of the natural redox partner, O₂, by the electrode; mediated bioelectrocatalysis was consistent with the potentials of a soluble redox mediator used. The results allow development of HOX-based electrochemical biosensors for sugar monitoring and biofuel cells exploiting direct ET of HOX, and, not the least, fundamental studies of ET non-complicated by the loss of FAD from the protein matrix.     

Direct electrodeposition of gold nanoparticles onto indium/tin oxide film coated glass and its application for electrochemical biosensor

A novel electrochemical deposition method for growth of gold nanoparticles (GNPs) on indium tin oxide (ITO) thin film coated glass was investigated. The resulting electrode surface was characterized by SEM, UV–Vis spectroscopy and electrochemical methods. The GNPs directly attached on the electrode surface with a quasi-spherical shape and their sizes of diameters were in the range of 20–35 nm with a quite symmetric distribution. With increasing electrodeposition cycles of cyclic voltammetry, the density of GNPs on ITO electrode surface was increased. The potential utility of the GNPs modified ITO electrode was investigated. Superoxide dismutase (SOD) was successfully immobilized on GNPs modified ITO electrode and the direct electron transfer between enzyme and electrode surface realized. The enzyme electrode exhibited a rapid and high response to superoxide anion.     

Direct electrochemistry of glucose oxidase on a graphite nanosheet–Nafion composite film modified electrode

The direct electrochemistry of glucose oxidase (GOD) immobilized in a modified electrode based on a composite film of exfoliated graphite nanosheets (GNSs) and Nafion has been investigated for the first time. Direct electron communication between GOD and the electrode was achieved with a fast electron transfer rate (12.6 s^?1). In addition, the bioactivity of GOD was retained after immobilization in the composite film and glucose could be determined based on the decrease of the electrocatalytic response of the reduced form of GOD to dissolved oxygen. The resulting biosensor exhibited higher sensitivity (3.4 μA mM^?1). Considering much lower cost of GNSs and ready preparation from graphite, the GNSs-based modified electrode described here is superior to the carbon nanotubes (CNTs)-based modified electrodes and should have wide applications in third-generation biosensors, bioelectronics and electrocatalysis.     

Bioelectrocatalytic current based on direct heterogeneous electron transfer reaction of glucose oxidase adsorbed onto multi-walled carbon nanotubes synthesized on platinum electrode surfaces

Multi-walled carbon nanotubes (MWCNTs) were synthesized on platinum plate electrodes by the chemical vapor deposition (CVD) method. The MWCNTs synthesized on the Pt plate (MWCNTs/Pt) electrode were immediately immersed into solutions of glucose oxidase (GOX) to immobilize these enzymes onto the MWCNTs/Pt electrode surfaces. After the GOX was immobilized onto the MWCNTs/Pt electrode, a well-defined catalytic oxidation current was increased from ca. −0.45 V (vs. Ag/AgCl/saturated KCl), which was close to the redox potential of flavin adenine dinucleotide (FAD) as a prosthetic group of GOX under physiological pH values.     

Direct electrochemical response of cytochrome c on a room temperature ionic liquid,N-butylpyridinium tetrafluoroborate,modified electrode

Cytochrome c (Cyt c) and a room temperature ionic liquid (RTIL), 2-methyl-N-butylpyridinium tetrafluoroborate ([2-MBPy][BF₄]), were immobilized on the surface of a basal plane graphite (BPG) electrode. Direct electron transfer from Cyt c to BPG electrode was clearly observed. A pair of well-defined and reversible redox peaks could be obtained in a 0.13 M [2-MBPy][BF₄] aqueous solution. The anodic and cathodic peak potentials of Cyt c were at −0.064 and −0.020 V (vs. Ag/AgCl), respectively. The results showed that [2-MBPy][BF₄] promoted the direct electron transfer between Cyt c and the BPG electrode. Cyt c immobilized on BPGE can catalyze the reduction of hydrogen peroxide. Based on this, a biosensor can be constructed to detect quantitatively hydrogen peroxide.     

A microfluidic glucose biofuel cell to generate micropower from enzymes at ambient temperature

A Y-shaped microfluidic channel is applied for the first time to the construction of a glucose/O₂ biofuel cell, based on both laminar flow and biological enzyme strategies. During operation, the fuel and oxidant streams flow parallel at gold electrode surfaces without convective mixing. At the anode, the glucose oxidation is performed by the enzyme glucose oxidase whereas at the cathode, the oxygen is reduced by the enzyme laccase, in the presence of specific redox mediators. Such cell design protects the anode from an interfering parasite reaction of O₂ at the anode and offers the advantage of using different streams of oxidant and fuel for optimal performance of the enzymes. Electrochemical characterizations of the device show the influence of the flow rate on the output potential and current density. The maximum power density delivered by the assembled biofuel cell reached 110 μW cm^?2 at 0.3 V with 10 mM glucose at 23 °C. The microfluidic approach reported here demonstrates the feasibility of advanced microfabrication techniques to build an efficient microfluidic glucose/O₂ biofuel cell device.