A Prospect for the Analysis of Species Acting as Enzyme Inhibitors as Illustrated by Heavy Metal Inhibition

Abstract

A flow system incorporating an amperometric glucose oxidase enzyme electrode has been used to study the inhibitory effects of 16 metal cations on glucose oxidase. Only copper(II), mercury(II) and silver(I) caused any significant inhibition. the enzyme electrode could be reactivated by EDTA, the reactivation being most effective for copper(II) and least so for silver(I). Other complexing agents were tried for reactivation but proved to be unsatisfactory.

The ability to reactivate the enzyme on the electrode following copper(II) inhibition, and the linear response of the system to the level of this inhibitor according to I/A = -9.49 × 10^?7 log([Cu]/M) + 4.84 × 10^?8; r = 0.994 between 2.5 × 10^?4M and 5 × 10^?3M [Cu]²⁺ indicates a prospect for the use of a flow system for determining enzyme inhibitors in samples.     

Amperometric Glucose Biosensor Based on the Deposition of Copper and Glucose Oxidase onto Glassy Carbon Transducer

ABSTRACT

The performance of a first generation glucose amperometric biosensor based on the entrapment of glucose oxidase (GOx) within a net of copper electrodeposited onto activated glassy carbon electrode, is described. The copper electrodeposited offers an efficient electrocatalytic activity towards the reduction of enzymatically-liberated hydrogen peroxide, allowing for a fast and sensitive glucose quantification. The influence of the electrodeposition conditions (pH, potential, time, copper salt and enzyme concentrations) on the response of the bioelectrode was evaluated from the amperometric signals of hydrogen peroxide and glucose. The combination of copper electrodeposition with a nation membrane allows an excellent selectivity towards easily oxidizable compounds such as uric and ascorbic acids at an operating potential of -0.050 V. The response is linear up to 2.0 × 10^?2 M glucose, the detection limit being 1.2 × 10^?3 M.     

Development of a Novel Silver Nanoparticles-Enhanced Screen-Printed Amperometric Glucose Biosensor

Abstract

A disposable glucose biosensor is developed by immobilizing glucose oxidase into silver nanoparticles-doped silica sol-gel and polyvinyl alcohol hybrid film on a Prussian blue-modified screen-printed electrode. The silver nanoparticles-enhanced biosensor shows a linear amperometric response to glucose from 1.25 × 10^?5 to 2.56 × 10^?3 with a sensitivity of 20.09 mA M^?1 cm^?2, which is almost double that of the biosensors without silver nanoparticles. The immobilized glucose oxidase retained 91% of its original activity after 30 days of storage in phosphate buffer (pH 6.9; 0.1 M) at 4°C. Blood glucose in a rabbit serum sample was successfully measured with the biosensor.     

Chitosan‐Based Glucose Oxidase Electrodes Enhanced by Silver Nanoparticles

Silver nanoparticles enhanced glucose oxidase electrodes were prepared on the basis of chitosan matrix. The enzyme electrodes exhibited high sensitivity and excellent response performance to glucose with a linear range from 1×10^?6 to 8×10^?3 mol · L^?1. And the time reaching the steady‐state amperometric response was less than 5 seconds. The inhibition percentage of this enzyme electrode against copper ions concentration was linear ranging from 1.2×10^?6 to 5×10^?5 mol · L^?1. These properties of enzyme electrodes are probably due to the excellent electron transfer of silver nanoparticles and the orientation of glucose oxidase molecule.     

New Potentiometric Membrane Sensors Responsive to Pb(Ii) Based on Some Recently Synthesized 9, 10- Anthraquinone Derivatives

ABSTRACT

New potentiometric membranesensorsresponsive to Pb(II) have been developed. The membrane sensors are based on three different 9, 10-anthraquinone derivatives. The electrode based on 1, 4-bis (prop-2¹-enyloxy)-9, 10-anthraquinone exhibits a good Nernstian response for Pb(II) ions over a wide concentration range (2.5×10^?6 - 1.0×10^?2 M) with a slope of 29.8 mV decade^?1. Detection limit is 1.5×10^?6 M. The response time of the sensor is 15s and the useful working pH range is 4.7-6.8. The membrane can be used for more than 4 months without any considerable divergence in potentials. The electrodes revealed comparatively good selectivities with respect to alkali, alkaline earth and some transition and heavy metal ions. It was used as an indicator electrode in potentiometric titration of lead ions (with sulfate and oxalate ions), and for the determination of lead in waste waters.     

Micro-Enzyme Electrode Prepared on Platinized Platinum

Abstract

Micro-enzyme electrode with high performance was fabricated on a micro-platinum electrode surface (diameter = 50 ～ 200 μm) by taking advantage of very huge surface of platinized platinum. Glucose oxidase was incorporated into the micropores of platinum particle by immersing a micro-platinized platinum electrode in a solution containing glucose oxidase. The micro-enzyme electrode for glucose demonstrated high performance such as high sensitivity (the least detectable limit : 5 × 10^?7 M), fast responsiveness (100 % response : 3 sec), and accuracy (C.V. = 1.4 %) in the repeated determination of glucose.     

Amperometric Biosensors Based on Platinum Nanowires

Abstract

Platinum nanowires (PtNW) were prepared by an electrodeposition strategy using nanopore alumina template. The nanowires prepared were dispersed in chitosan (CHIT) solution and stably immobilized onto the surface of glassy carbon electrode (GCE). The electrochemical behavior of PtNW‐modified electrode and its application to the electrocatalytic reduction of hydrogen peroxide (H₂O₂) are investigated. The modified electrode allows low potential detection of hydrogen peroxide with high sensitivity and fast response time. As an application example, the glucose oxidase was immobilized onto the surface of PtNW‐modified electrode through cross‐linking by glutaric dialdehyde. The detection of glucose was performed in phosphate buffer at –0.2 V. The resulting glucose biosensor exhibited a short response time (<8 s), with a linear range of 10^?5?10^?2 M and detection limit of 5×10^?6 M.     

Comparative study of potentiometric and amperometric tissue-based electrodes for oxalate

Acetone-precipitated pulp from banana skins is physicall entrapped at the tip of a carbon dioxide gas-sensor and on a hydrogen peroxide sensor probe to determine oxalate potentiometrically and amperometrically in aqueous solution and inurine. The enzyme present in the tissue is oxalate oxidase. The potentiometric response has a slope of 47–50 mV/decade for 1 × 10^?4 M–2 × 10^?3 M oxalate with a detection limit of 2 × 10^?5 M. The amperometric response is linear for 2 × 10^t-5–3 × 10^?4 M oxalate with a dectection limit of 2 × 10^?6 M. Average recoveries of oxalate added to aqueous samples were 96.2% and 98.0%, and average relative standrd deviations were 3.8% and 3.6% for the potentiometric and amperometric systems, respectively. Oxalate was determined in six control urine samples, with relative errors of about 2.5%, by both electrode systems after a simple clean-up.     

Glucose Oxidase Electrode Based on Graphite and Methylthio Tetrathiafulvalene as Mediator

Abstract

A glucose sensor based on glucose oxidase and a new mediator - 4,5-dimethyl-4′-methylthio-Δ 2,2′-bi-1,3-dithiole (MTTTF) is described. The background for sensor action is the effective MTTTF cation interaction (apparent bimolecular constant (2.0+/-0.5)?10⁶ M^?1 s^?1 at 25°C and pH 7.0) with reduced glucose oxidase and the high electrochemical rate of mediator transformation.

A glucose sensor was prepared by adsorbing mediator (MTTTF) and glucose oxidase on graphite rods. The sensor responds to glucose at electrode potentials higher than 50 mV vs SCE, but the maximal activity is obtained at a potential of 250 mV. In air saturated solution the electrode shows a non-linear calibration curve with a half-saturation concentration 10.4 mM and Hill coefficient 2.08 at 250 mV. Sensor response changes little at pH 6.5–8.0. The energy of activation of the sensor response calculated from the Arrhenius equation was 64.5 kJ/mol, and the temperature coefficient at 25°C was 9.2%.     

Development and Application of an Immobilized Enzyme Electrode for the Determination of Sulfite in Foods and Feeds

Abstract

An enzyme electrode was developed using the enzyme sulfite oxidase (EC 1.8.3.1) immobilized onto pig intestine. All experimental parameters such as pH, temperature, buffer constituent concentration, etc., were thoroughly investigated and optimized when appropriate. Hydrogen peroxide was monitored amperometrically. The response to sulfite concentration was linear in the range of 5.2 × 10^?6 to 1.0×10^?3M. The proposed method was found to have a correlation coefficient of 0.952 when evaluated versus the standard titration method.     

Detection of Oxidase Generated Hydrogenperoxide by a Solid State Peroxyoxalate Chemiluminescence Detector

Abstract

The compatability of a solid state peroxyoxalate chemiluminescence detector for hydrogen peroxide with an immobilized oxidase reactor is investigated. As a model system glucose oxidase immobilized by electrostatic forces on an ion-exchanger or chemically bonded to glass beads were chosen. The former support is less suitable for immobilization of oxydases due to strong retention of hydrogenperoxide on the ion exchanger.

The relatively little flow dependence of these systems renders them suitable for low-cost manual sample injection monitors as well as in a flow injection analyses (FIA) mode with low-cost pumping systems. The system was operated with 80% acetonitrile water solutions. A detection limit of 8 × 10^?7M of glucose was achieved in directly injected samples.

Enzymes more sensitive to organic solvents can be operated with pure water and adjustment for optimal chemiluminescence condition is achieved with a make-up flow prior to detection. A detection limit of 5 × 10^?8M glucose is achieved under these conditions. The feasability of this approach to other oxidase based monitors and to detection in liquid chromatography is discussed.     

A Fast Made Disposable Glucose Biosensor Incorporating the Oxidase and a Ferrocene in an Alginate Gel

Abstract

A simple procedure is described for co-immobilization of glucose oxidase and dimethylaminomethylferrocene in a sodium alginate gel on the surface of pyrolytic graphite electrode. The film is electrochemically active and the peak current is a function of D-glucose concentration with the apparent Michaelis-Menten constant K_m = (1.2±0.3) × 10^?2 M. The optimal concentration range for biosensoric applications in 0.001–0.010 M.

     

Construction and Characterization of a Beet Stem Based Biosensor for Oxalate

Abstract

This report describes the construction and characterization of an oxalate-sensing electrode. The electrode is based on the incorporation of ground beet stem into the graphite paste of a graphite paste electrode. The hydrogen peroxide generated by enzymatic degradation of oxalate is monitored at a working voltage of 0.900 V vs SCE. All measurements were conducted in a succinic acid/EDTA buffer at pH 4.00. Under these conditions, the electrodes exhibit reproducible responses to oxalate. The lower limit of oxalate detection was less than 1.03 × 10^?4 M. The time to achieve a steady state response after exposure to a step change in oxalate concentration in solution is less than one minute. The magnitude of response to oxalate over the oxalate concentrations studied varies among several electrode tested as does the degree of linearity of response. An electrode studied still exhibited analytically useful responses to oxalate on the 15th day of its use. The beet stem-based electrodes display little response to glycolic acid, glucose, DL-valine, or pyruvate.     

Bienzyne Electrodes for ATP,NAD+, Starch and Disaccharides Based on a Glucose Sensor

Abstract

A glucose measuring device based on the oxidation of glucose by glucose oxidase and an amperometric kinetic detection was developed. The characteristics obtained with this instrument are comparable with the present glucose instruments but the stability of the enzyme membrane is better and the measuring frequency is higher. In order to expand the applicability of this device to other substrates there was developed a family of bioenzyme electrodes. Enzymes producing glucose as enzymes consuming glucose in addition to glucose oxidase were used.

For determination of peroxidase substrates besides a peroxidase-catalase electrode a three-enzyme system consisting of glucose oxidase, peroxidase and catalase was used.     

Electrode Hybride Pour la Determination de Phosphates et de Polyphosphates. Application aux Problemes Lies a l'Environnement

Abstract

The determination of phosphates and polyphosphates has been effected using an hybrid electrode, which consists of a glucose oxydase enzymic membrane and a Solanum tuberosum tissue slice. This membrane, rich in acid phosphatase, catalyses the glucose-6-phosphate hydrolysis. This reaction is quantitatively inhibited by phosphate. Several factors involved in the electrode response, like substrate concentration, pH, ionic strength and type of buffer are discussed in detail. At a 4.10^?4 M glucose-6-phosphate concentration, the linear ranges of phosphates and polyphosphates are, respectively, 6.10^?5 M to 1.6.10^?3 M and 3.10^?5 M to 1.10^?3 M. The urinary phosphate contents determinated by this biosensor are in good agrement with those obtained by usual spectrophotometric techniques.     

Construction of a N-Acetyl-L-methionine Electrode and Determination of Acylase with an Ammonia Gas Sensor

Abstract

The N-acetyl-L-methionine electrode is based on a coupled enzymatic system consisting of acylase and L-amino acid oxidase with an ammonia gas sensor; conditions of imobilization are optimized. N-acetyl-L-methionine in the range 4×10^?5–2×10^?3M gives a linear potential vs. log(concentration) plot with a response time of 2–5 min over the range specified. This electrode combined with an L-methionine electrode, based only on L-amino acid oxidase and an ammonia gas sensor, can be used for the determination of both substrates in mixtures, thus extending the feasibility of the method. Acylase (0.1–2.00) is determined in aqueous solutions by adding N-acetyl-L-methionine to the sample, and measuring the ammonia evolved with the gas-sensing electrode.     

Electrochemical Behaviour of a Lipid Modified Enzyme Electrode

Abstract

The modification of the surface of a platinum electrode by coating with a layer of a lipid mixture (asolectin), allows the relative measurement of hydrogen peroxide in the presence of interfering analytes. The lipid-enzyme complex and the platinum amperometric sensor offer greater selectivity and extended stability of the resulting probe. Measurements of glucose with the glucose oxidase enzyme and detection of the liberated hydrogen peroxide have been performed as a model system. Linear response of the signal versus glucose concentration was observed in the range of glucose concentration 1.10^?3 ? 1.10^?5 M with a response time of 20 s. The interferences of ascorbic acid, uric acid, iron (II), paracetamol, tyrosine and glutathion can be drastically minimized by appropriate adjustment of the amount of lipid contained in the biocatalyst layer.     

Solid Membranes of Copper Hriacyanoferrats (III) as Thallium (I) Sensitive Electrode

Abstract

Solid membranes of copper hexacyanoferrate (III) in Areldite are evaluated as thallium (I) sensitive electrode. The membrane electrode gave a linear near Normstian response to thallium (I) ions in the concentration range 10^?1 - 5 × 10^?4 M and can be used to estimate T1 (I) down to 10^?4 M. The responses of the electrode is fast and steady potentials are obtained in less than a minute. The same membrane has been used over a period of six months without any appreciable drift in potential. The electrode can also be used satisfactory in partially non-aqueous media and in presence of a number of interfering ions. It is superior to the existing T1(I) solid membrane electrodes as it can function in alkaline range also.     

Amperometric determination of glucose in undiluted food samples

Glucose oxidase is immobilized onto a cellulose acetate membrane by glutaraldehyde linkage, and the membrane is used to cover the platinum electrode of a hydrogen peroxide sensor. A silanized polycarbonate membrane then covers the enzyme layer, and extends the linear calibration range to higher concentrations. The sensor, when incorporated into a flow-injection system, allows the determination of glucose at levels up to 1 M in soft drinks at a rate of 60 samples h^?1 without sample dilution.     

Phosphate-sensitive enzyme electrode: a potential sensor for environment control

A highly sensitive enzyme electrode was designed for the assay of phosphate ions. For this purpose, a bienzyme membrane with co-immobilized nucleoside phosphorylase and xanthine oxidase was used with a platinum amperometric electrode for the detection of enzymatically generated hydrogen peroxide. A detection limit of 10^?7 M was obtained and phosphate assays could be easily performed in the range 0.1–10 μM, which is of interest in the control of water pollution.