Microfluidic cell arrays for metabolic monitoring of stimulated cardiomyocytes

An array of PDMS microchambers was aligned to an array of sensor electrodes and stimulating microelectrodes, which was used for the electrochemical monitoring of the metabolic activity of single isolated adult ventricular myocytes inside the chamber array, stimulated within a transient electric field. The effect of the accumulation of metabolic byproducts in the limited extracellular volume of the picolitre chambers was demonstrated by measuring single muscle cell contraction optically, while concomitant changes in intracellular calcium transients and pH were recorded independently using fluorescent indicator dyes. Both the amplitude of the cell shortening and the magnitude of the intracellular calcium transients decreased over time and both nearly ceased after 20 min of continuous stimulation in the limited extracellullar volume. The intracellular pH decreased gradually during 20 min of continuous stimulation after which a dramatic pH drop was observed, indicating the breakdown of the intracellular buffering capacity. After continuous stimulation, intracellular lactate was released into the microchamber through cell electroporation and was detected electrochemically at a lactate microbiosensor, within the chamber. A mitochondrial uncoupler was used to mimic ischaemia and thus to enhance the cellular content of lactate. Under these circumstances, intracellular lactate concentrations were found to have risen to ～15 mM. This array system has the potential of simultaneous electrochemical and optical monitoring of extracellular and intracellular metabolites from single beating heart cells at a controlled metabolic state.     

Ultra-simple adaptor to convert batch cells with mercury drop electrodes in voltammetric detectors for flow analysis

A simple, robust and fast-responding flow adaptor for mercury drop electrodes (MDEs) is described. An L-shaped PTFE tube with an internal diameter of 0.5 mm is fixed with a silicone ring on the glass capillary of a MDE, in such a way as to direct the outcoming flow onto the mercury drop, from a distance of about 0.5 mm. Any commercial or laboratory-made batch cell, provided with an MDE, serves for the purpose. The level of supporting electrolyte in the cell is maintained constant through a siphon or a lateral draining orifice. The adaptor is compatible with all the different brands and operating modes of the MDEs (free dropping, controlled drop time, renewable static drop, hanging drop or sessile drop). Flow injection experiments were conducted with the following amperometric detection modes: sampled-DC, reverse pulse amperometry (RPA), and anodic stripping voltammetry (ASV). The FIA-RPA peaks presented a R.S.D.<0.8% for 1.0×10⁻⁵ mol l⁻¹ lead(II) (N=30, V_sample=100 μl). The response time (0-63% of the signal maximum) to a concentration step is 1.2 s for 500 μl injections of 0.1 mmol l⁻¹ ascorbic acid in acetate buffer at a flow rate of 1 ml min⁻¹, which corresponds to a response volume of 20 μl. As an example of practical application, copper(II) was determined in fertilizers by RPA using the standard addition method, at an analytical frequency of 90 injections per h.     

Comparison of metallic electrodes for constant-potential amperometric detection of carbohydrates,amino acids and related compounds in flow systems

Constant-potential amperometric detection of carbohydrates, amino acids, and other aliphatic organic compounds is possible by means of their oxidation in alkaline solution at a variety of metal/metal oxide electrodes including Pt, Au, Cu, Ni, Ag and Co. The experimental conditions required for optimum detection and the analytical performance obtainable vary widely for different electrode materials and analytes. In this work, the cyclic voltammetric behavior exhibited by selected analytes (glucose, glycine, lactic acid, ethylamine and ethanol) at each of these electrodes was used to determine the optimum potentials suitable for flow detection so that the capabilities of the different metal electrodes could be evaluated and systematically compared. In general, the Cu electrode was found to provide superior detection capabilities in terms of its range of response, detection limits and especially stability. Despite the fact that Pt and Au are typically used only with a pulsed applied potential, both can provide long-lived constant-potential detection of carbohydrates and other analytes at low concentrations if the potentials ere carefully chosen and the electrodes are allowed to undergo an initial stabilization period.     

Amperometric glucose sensor using tetrathiafulvalene in Nafion gel as electron shuttle

An amperometric mediated sensor for glucose has been contrived by using bovine serum albumin and glutaraldehyde to immobilize glucose oxidase on a Nafion-tetrathiafulvalene (TTF) modified electrode. It is further coated by Nafion. The inner Nafion membrane can prevent leaking of tetrathiafulvalene; the outer Nafion film serves as a barrier to electroactive anionic interferents such as ascorbate and urate and protects the biosensor from fouling agents. The experiment shows that TTF⁺ and TTF²⁺ can oxidize the reduced flavin adenine dinucleotide (FADH₂) of glucose oxidase. The biosensor responds to glucose in less than 50 s and its calibration curve is linear from 3.0 × 10⁻⁴ to l.0 × 10⁻² M.     

Donnan dialysis preconcentration coupled with ion chromatography and electrocatalytic oxidation for the determination of cyanide

An electrocatalytic amperometric detector for the ion chromatographic determination of CN⁻ is described. A conducting composite that is based on a graphite-loaded sol–gel material comprises the working electrode. The composite is doped with a Ru^II metallodendrimer which is demonstrated to promote the electrochemical oxidation of CN⁻ at potentials positive of 0.5 V vs. Ag/AgCl. In 6 mM NaOH, 0.05 M NaCl flowed at 1.0 ml min⁻¹, a 5-point calibration curve with the following linear least squares parameters is obtained over the range, 1.0–30 M CN⁻: slope, 24.2±0.1 nA M⁻¹; intercept, −6±2 nA; and r, 0.9997. The detection limit, 0.7 μM CN⁻, compares favorably to that obtained by amperometry at a silver electrode, 0.5 μM CN⁻, under comparable experimental conditions. A 60-min preconcentration by Donnan dialysis increases the sensitivity by a factor of 23.6.     

Preparation of Ce-PbO(2) modified electrode and its application in detection of anilines

The effect of Ce(III) on the morphology and structure of lead dioxide (PbO₂) modified electrode was studied in this paper. The results obtained by cyclic voltammetry (CV), X-ray diffractometion (XRD) and scanning tunneling micrograph (STM) indicated that the Ce-doped PbO₂ film consisted of a mixture of α- and β-PbO₂ crystallographic phases and the content of α-phase was higher than that in undoped PbO₂ film. PbO₂ crystal grains in nanometric size were formed on the electrode surface by doping with Ce. So that the specific surface areas and catalytic active sites of the modified electrode were increased. Hence the catalytic activity of the Ce-PbO₂ modified electrode was evidently greater than the undoped PbO₂ modified electrode. When the Ce-PbO₂ modified electrode was applied as an analytical sensor to determine aniline compounds, the linearity was in the range of 5×10⁻⁵ to 1×10⁻³ mol/l and the detection limit was 1×10⁻⁵ mol/l.     

Characterization of graphite electrodes modified with laccase from Trametes versicolor and their use for bioelectrochemical monitoring of phenolic compounds in flow injection analysis

Spectrographic graphite electrodes were modified through adsorption with laccase from Trametes versicolor. The laccase-modified graphite electrode was used as the working electrode in an amperometric flow-through cell for monitoring phenolic compounds in a single line flow injection system. The experimental conditions for bioelectrochemical determination of catechol were studied and optimized. The relative standard deviation of the biosensor for catechol (10 μM, n=12) was 1.0% and the reproducibility for six laccase-modified graphite electrodes, prepared and used different days was about 11%. The optimal conditions for the biosensor operation were: 0.1 M citrate buffer solution ( at pH 5.0), flow rate of 0.51 ml min⁻¹ and a working potential of −50 mV versus Ag|AgCl. At these conditions the responses of the biosensor for various phenolic compounds were recorded and the sensor characteristics were calculated and compared with those known for biosensors based on laccase from Coriolus hirsutus, cellobiose dehydrogenase (CDH) from Phanerochaete chrysosporium and horseradish peroxidase (HRP).     

Amperometric determination of oxidizable solutes in water with a solution exchange technique

Determination of oxidizable solutes in water is accomplished using amperometric detection in a solution exchange apparatus. The applied potential (E_a) used is + 0.5 V vs. SCE at a nickel working electrode. Electrode pretreatment is performed at −1.0 V vs. SCE. The background electrolyte is 0.1 M NaOH. Analyte solution drawn into the cell replaces background solution. No further convection occurs. Peak anodic current relative to the baseline is used as the analytical signal. The linear range extends down to 1 μM for sucrose, diethylenetriamine, phenol, and ethanolamine. The determination time is 2 min per sample.     

Silicate electrochemical measurements in seawater: Chemical and analytical aspects towards a reagentless sensor

From the study of molybdenum oxidation in aqueous solutions we developed a semi-autonomous method to detect silicate in aqueous samples. Molybdenum oxidation was used to form molybdate in acidic media. The silicomolybdic complex formed with silicate is detectable by amperometry or cyclic voltammetry. The new electrochemical method is in good agreement with the method conventionally used for environmental water silicate analysis. In the second stage, a completely reagentless method was developed using molybdate and proton produced during molybdenum oxidation. Reproducibility tests show a precision of 2.6% for a concentration of 100 μmol L⁻¹. This new method will be very suitable for the development of new autonomous silicate sensors easy to handle and without reagents. In this paper we present the analytical and chemical aspects necessary for a complete documentation of the method before the development of a new reagentless sensor.     

Development of an amperometric immunosensor based on flow injection analysis for the detection of red blood cells

An amperometric immunosensor, based on a non-competitive sandwich assay and flow injection analysis (FIA), was developed for the detection of human red blood cells (RBCs). A dual working electrode, on which specific IgM and nonspecific IgM were chemically immobilised to form sensing and blank electrodes, respectively, was employed to determine the binding of specific blood cells and non-specific adsorption in one determination. Horseradish peroxidase (HRP)-labelled antiblood group A IgM was used in the assay. Sensor preparation involved chemical immobilisation of the IgMs on glassy carbon electrodes using l-ethyl-3(3-dimethyl aminopropyl)carbodiimide (EDC) as a coupling reagent in the presence of N-hydroxysuccinimide (NHS). The interference contributions, such as the non-specific adsorption of the enzyme conjugate and the blood cells, were determined and removed. A quantitative relationship between the cell binding response and its concentration was obtained in the region 1 − 30 × 10⁸ cells ml⁻¹.