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.     

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.     

Pure copper vs. mixed copper and palladium hexacyanoferrates for glucose biosensing applications

A glucose amperometric biosensor was developed. Glucose oxidase enzyme was immobilized by means of a Nafion membrane on glassy carbon modified with an electrochemically deposited mixed Cu and Pd hexacyanoferrate (CuPdHCF). According to the data provided by X-ray atomic spectroscopy measurements, this Cu- and Pd-based hexacyanoferrate is likely to be a mixture of single CuHCF and PdHCF pure phases. The biosensor performances were evaluated by recording the steady-state currents due to submillimolar additions of glucose to a potassium buffer solution (pH 5.5) and exploiting the electrocatalytic reduction of the enzymatically produced hydrogen peroxide. The CuPdHCF-based biosensor exhibited a sensitivity of 8.1?±?0.6 A M^?1 m^?2, a limit of detection of 1.4?×?10^?5 M, and a linear response range extending between 5?×?10^?5 and 4?×?10^?4 M, with a dynamic response range up to 4?×?10^?3 M glucose. Electrode sensitivity and signal stability resulted more satisfactory as compared to those of a CuHCF-based biosensor fabricated according to the same procedure. The selectivity was investigated through an interference study. The response to easily oxidizable species was found to be low enough to allow glucose determination in biological samples.     

Amperometric Glucose Biosensor Based on Platinum Nanoparticles Combined Aligned Carbon Nanotubes Electrode

A sensitive amperometric glucose biosensor based on platinum nanoparticles (PtNPs) combined aligned carbon nanotubes (ACNTs) electrode was investigated. PtNPs which can enhance the electrocatalytic activity of the electrode for electrooxidating hydrogen peroxide by enzymatic reaction were electrocrystallized on 4‐aminobenzene monolayer‐grafted ACNTs electrode by potential‐step method. These PtNPs combined ACNTs' (PtNPs/ACNTs) surfaces were characterized by scanning electron microscopy (SEM) and transmission electron microscopy (TEM). The highly dispersed PtNPs on ACNTs can be obtained. The enzyme electrode exhibits excellent response performance to glucose with linear range from 1×10^?5–7×10^?3 mol L^?1 and fast response time within 5 s. Furthermore, this glucose biosensor also has good reproducibility. It is demonstrated that the PtNPs/ACNTs electrode with high electrocatalytic activity is a suitable basic electrode for preparing enzyme electrodes.     

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.     

Determination of Damaged Starch in Wheat Flour Using an Electrochemical Bienzyme Maltose Probe

Abstract

The development of an electrochemical biosensor based on a bienzyme maltose probe and a third enzyme α-amylase in solution is reported for the rapid and inexpensive determination of damaged starch. Analytical parameters, such as probe stability, pH, temperature and response time, were optimised. Damaged starch was measured in the range of 5 × 10^?6 - 5 × 10^?4 mol/L as maltose produced by the enzymatic reaction and the detection limit was calculated according with the free maltose and/or glucose in the sample. The damaged starch was determined in different wheat flours, and the data significantly correlated with those obtained using a reference procedure (r² = 0.994; P ≤ 0.0001). In addition the results showed a comparable precision (CV < 5%). This method is rapid, inexpensive and friendly for unskilled operators.     

Flow-Injection Determination of Glucose by a Photoinduced Chemiluminescent Reaction

Abstract

A flow-injection procedure for the photochemical determination of glucose has been developed. The method is based on the photo-oxidation of glucose sensitized by 9,10-anthraquinone-2.6-disulfonate (disodium salt). The hydrogen peroxide formed in the photochemical reaction was measured by means of the chemiluminescent reaction with luminol and hematin. A linear calibration graph was obtained over the range 2.0x10^?6-8.5 x 10^?5 mol L^?1. The method was applied to determining glucose in blood serum, urine and fruit juices.     

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.     

铜（II）离子对脱镁叶绿素-a荧光猝灭的研究

本文介绍了一种利用荧光熄灭定量的测定铜（II）的新方法。从新鲜菠菜中提取叶绿素-a,用高氯酸溶液处理,制得脱镁叶绿素-a。测量脱镁叶绿素-a的紫外-可见吸收光谱,观测到505和535nm处有特征吸收峰。在60 ℃水浴中,脱镁叶绿素-a的丙酮溶液与铜（II）离子水溶液混合,5分钟后发现混合液颜色变绿,505和535 nm处吸收峰消失。铜（II）离子水溶液与脱镁叶绿素-a的丙酮溶液混合后发生荧光猝灭现象,而类似浓度的其它生理离子在相同反应条件下对脱镁叶绿素-a的荧光猝灭现象不明显。 研究了铜（II）离子与脱镁叶绿素-a的反应时间,反应温度对荧光强度衰减的影响。并通过阿累尼乌斯经验关系估算铜（II）离子与脱镁叶绿素-a反应的活化能约为10 ±1kJ·mol-1。研究了铜（II）离子的浓度对脱镁叶绿素-a的丙酮溶液荧光强度的影响,在8.0×10-5 ～8.0×10-7 mol·dm-3范围内,铜（II）离子的浓度与混合液的荧光强度成线性衰减关系,检测限可达8.0×10-7 mol·dm-3。利用脱镁叶绿素-a的丙酮溶液的荧光强度变化测量,有望发展成为一种检测铜（II）离子的新方法。     

Indirect determination of iron in a flow-injection system with amperometric detection

The change in peak current resulting from the reaction of Fe(II) with nitroso-R salt in a flow-injection system is used to quantify Fe(II) with either single- or dual-electrode amperometric detectors. The current change varies linearly with Fe(II) concentration from 0 to 200 mg 1^?1. The relative standard deviation was about 5% with the single-electrode detector and about 10% with the dual-electrode detector. The method is evaluated for the determination of iron in dietary supplements.     

Supramolecular immobilization of glucose oxidase on gold coated with cyclodextrin-modified cysteamine core PAMAM G-4 dendron/Pt nanoparticles for mediatorless biosensor design

Cysteamine core polyamidoamine G-4 dendron branched with β-cyclodextrins was chemisorbed on the surface of Au electrodes and further coated with Pt nanoparticles. Adamantane-modified glucose oxidase was subsequently immobilized on the nanostructured electrode surface by supramolecular association. This enzyme electrode was used to construct a reagentless amperometric biosensor for glucose, making use of the electrochemical oxidation of H₂O₂ generated in the enzyme reaction. The amperometric response of the biosensor was rapid (6 s) and a linear function of glucose concentration between 5 and 705 μmol?L^?1. The biosensor had a low detection limit of 2.0 μmol?L^?1, sensitivity of 197 mA?mol^?1?L?cm^?2, and retained 94 % of its initial response after storage for nine days at 4 °C.     

Horseradish Peroxidase Enzyme Electrodes for Nadh and Nadph

Abstract

The aerobic oxidation of reduced pyridine phosphonucleotides catalyzed by horseradish peroxidase (E.C.1.11.1.7) (HRP) in combination with Mn²⁺-ions, phenolics and redox dyes was used to perform NADH and NADPH determinations with an amperometric HRP enzyme electrode. Optimal operational conditions have been elaborated for such a sensor and a linear relationship between derivative current (dI/dt) and NADH-concentration was obtained between 2.10^?5 and at least 2.10^?4 mol/l. The coefficient of variation was equal to or smaller than 4 %. The time for one measurement was less than 10 minutes including equilibration of the electrode.     

Flow Injection Photoamperometric Investigation of Ascorbic Acid Using Methylene Blue Immobilized on Titanium Phosphate

Abstract

Methylene blue (MB) was incorporated into titanium phosphate (TiP) after pretreatment of TiP with the gas, n‐butyl amine. The dye is strongly retained and not easily leached from the layered host matrix. The adsorbed MB on TiP was used to prepare modified carbon paste electrodes (MCPE), which were studied voltammetrically and in amperometric flow injection (FI) mode for the electrocatalytic oxidation of ascorbic acid (AA). The electrochemical behavior of the immobilized dye was investigated with cyclic voltammetry, at a pH 7.0 phosphate buffer containing 0.5 M KCl, at different potential scan rates. The MB immobilized on the support underwent a quasi‐reversible electrochemical redox reaction. A homemade flow‐through electrochemical cell with a suitable transparent window for irradiation of the electrode surface was constructed and used for amperometric FI studies. The photoamperometric‐FI conditions were optimized for sensitivity and reproducibility at a flow rate of 1.5 mL/min, a transmission tubing length of 25 cm, a sample injection volume of 100 µL, and a constant applied potential of +100 mV vs. SCE. The calibration curve for AA was linear over the concentration range from 1.0×10^?6 to 2.5×10^?5 mol l^?1 for both amperometric and photoamperometric studies. But the slope of the photoelectrocatalytic FIA procedure was improved about 52% compared with those obtained without irradiation. The results obtained for AA determination in some pharmaceutical products are in good agreement with those obtained using the procedure involving the reaction between triiodide and AA.     

Hydrothermal Synthesis of Titanium‐Supported Nickel Nanoflakes for Electrochemical Oxidation of Glucose

Titanium‐supported nanoscale flaky nickel electrode (nanoNi/Ti) was prepared by a hydrothermal process using hydrazine hydrate as a reduction agent. Its electrocatalytic activity as an electrocatalyst for the electrooxidation of glucose was evaluated in alkaline solutions using cyclic voltammetry (CV), chronoamperometric responses (CA) and electrochemical impedance spectra (EIS). The nanoNi/Ti electrode exhibits significantly high current density of glucose oxidation. A high catalytic rate constant of 1.67×10⁶ cm³ mol^?1 s^?1 was calculated from amperometric responses on the nanoNi/Ti electrode. Low charge transfer resistances on the nanoNi/Ti in 0.5 M NaOH containing various concentrations of glucose were obtained according to the analysis for EIS. Furthermore, amperometric data show a linear dependence of the current density for glucose oxidation upon glucose concentration in the range of 0.05–0.6 mM with a sensitivity of 7.32 mA cm^?2 mM^?1. A detection limit of 0.0012 mM (1.2 μM) M glucose was found. Results show that the prepared nanoNi/Ti electrode presents high electrocatalytic activity for glucose oxidation.     

Development of urease based amperometric biosensors for the inhibitive determination of Hg (II)

Enzymatic amperometric procedures for measurement of Hg (II), based on the inhibitive action of this metal on urease enzyme activity, were developed. Screen-printed carbon electrodes (SPCEs) and gold nanoparticles modified screen-printed carbon electrodes (AuNPs/SPCEs) were used as supports for the cross-linking inmobilization of the enzyme urease. The amperometric response of urea was affected by the presence of Hg (II) ions which caused a decreasing in the current intensity. The optimum working conditions were found using experimental design methodology. Under these conditions, repeatability and reproducibility for both types of biosensors were determined, reaching values below 6% in terms of residual standard deviation. The detection limit obtained for Hg (II) was 4.2 × 10^?6 M for urease/SPCE biosensor and 5.6 × 10^?8 M for urease/AuNPs/SPCE biosensor. Analysis of the possible effect of the presence of foreign ions in the solution was performed. The method was applied to determine levels of Hg (II) in spiked human plasma samples.     

A Novel Enzyme Membrane Electrode for Oxalate Determination in Foodstuffs

Abstract

An enzyme membrane electrode usable for the assay of oxalate in foodstuffs is described. A commercially available preactivated polyamide membrane was used for the immobilization of oxalate oxidase. The bioactive disk thus obtained was associated with an amperometric transducer. The resulting self-contained enzyme electrode wich allows oxalate determination in various materials with minimal pretreatment exhibits a linear calibration ranging from 10–7 M and 10–4 M in the cell. The response-time was comprised between 20 seconds and 1 minute, depending on the oxalate content in the sample. The electrode-response was very stable for at least 4 months, a period during which more than 150 assays were performed.

The results obtained with several food materials were in good agreement with those obtained with the conventional spectrophotometric method. Assays were also performed with a microprocessor-based analyzer normally used for glucose measurements with a glucose oxidase electrode When the analyzer is equipped with an oxalate oxidase membrane, without further setting, oxalate can be determined in the range 5 10^?3 M-10^?1 M in the sample.     

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.     

Enzymes Immobilized on a Tubular Reactor for Fast Amperometric Determination of Glucose in Brazilian Honey

Abstract

Glucose present in honey was rapidly determined by the differential amperometric method using two tubular reactors containing glucose oxidase and peroxidase. The linear dynamic range extends from 5 × 10^?5 to 2 × 10^?4mol L^?1, at pH 7.0. At flow rate of 1.5 mL min^?1 and injecting 150-µL sample volumes, a sampling frequency of the 33 determinations per hour is afforded. The reproducibility of the methods showed a relative standard deviation (RSD) < 4%. The detection limit of this method is 1.7 × 10^?5 mol L^?1. The samples analyses were compared with the parallel spectrophotometric determination.     

一种基于壳聚糖固定葡萄糖氧化酶的葡萄糖生物传感器的研究

本文选用生物相容性好的壳聚糖作为基体材料，使其与戊二醛交联成网状结构包埋葡萄糖氧化酶制成电化学传感器。这种壳聚糖膜不仅可以减小葡萄糖氧化酶的流失，而且能为酶提供了适宜的微环境。用红外光谱、紫外光谱及透射电镜对膜的形态和性质进行了表征。实验结果表明该传感器具有很快的响应速度，很好的稳定性和重现性，能选择性地催化葡萄糖并测定其浓度。该传感器的制备方法简单，成本低，于冰箱中放置两周信号保持在90％以上，对葡萄糖测量的线性范围为1×10^-5 - 3.4×10^-3mol•L^-1，当信噪比为3:1时检测限为5×10^-6mol•L^-1。     

Biosensing of Aromatic Amines in Reversed Micelles with Self‐Generation of Hydrogen Peroxide at Glucose Oxidase‐Peroxidase Bienzyme Electrodes

The amperometric biosensing of aromatic amines using a composite glucose oxidase (GOD)‐peroxidase (HRP) biosensor in reversed micelles is reported. Rigid composite pellets of graphite and Teflon, in which GOD and HRP were coimmobilized by simple physical inclusion, were employed for the biosensor design. This design allows the in situ generation of the H₂O₂ needed for the enzyme reaction with the aromatic amines, thus preventing the negative effect that the presence of a high H₂O₂ concentration in solution has on HRP activity. The H₂O₂ in situ generation is performed by oxidation of glucose catalyzed by GOD. The effect of the composition of the reversed micelles, i.e., the nature of the organic solvent used as the continuous phase, the nature and concentration of the surfactant used as emulsifying agent, the aqueous 0.05 mol L^?1 phosphate buffer percentage used as the dispersed phase, and the glucose concentration in the aqueous phase, on the biosensor response was evaluated. Reversed micelles formed with ethyl acetate, a 5% of phosphate buffer (pH 7.0) containing 3.0×10^?3 mol L^?1 glucose, and 0.1 mol L^?1 AOT (sodium dioctylsulfosuccinate), were selected as working medium. Well‐defined and reproducible amperometric signals at 0.00 V were obtained for p‐phenylenediamine, 2‐aminophenol, o‐phenylenediamine, m‐phenylenediamine, 1‐naphthylamine, o‐toluidine and aniline. The useful lifetime of one single biosensor was of 60 days. The trend in sensitivity observed for the aromatic amines is discussed considering the effect of their structure on the stabilization of the radicals formed in the enzyme reaction which are electrochemically reduced. The behavior of the composite bienzyme electrode was also evaluated in a FI (flow injection) system using reversed micelles as the carrier. The suitability of the composite bienzyme electrode for the analysis of real samples was demonstrated by determining aniline in spiked carrots.