Enzymatic assay with detection by enhanced luminol chemiluminescence in a reversed micellar system: determination of l-amino acids and glucose

A detection system for hydrogen peroxide, i.e., luminol chemiluminescence (CL) in a hexadecyltrimethylammonium bromide (CTAB) reversed micellar system, was coupled to enzyme reactions. The use of CTAB reversed micellar medium allows one to conduct both the oxidase enzymatic and CL detection reactions simultaneously at mild pH (l-amino acid system, pH 8.7; glucose system, pH 8.5) in the absence of any co-oxidant or catalyst. Based on this result, simple and unique determinations of l-amino acids and glucose as substrates were developed. The calibration graph for a representative amino acid, l-phenylalanine, was linear in the concentration range 4.0×10^?6?200×10^?6M with a relative standard deviation of 5.78% (five determinations). The method established for l-phenylalanine was also applicable for the assay of fourteen other l-amino acids. The calibration graph for glucose was linear in the concentration range 5.4×10^??540×10^?6M with a relative standard deviation of 4.27% (eight determinations). This method was compared with a standard spectrophotometric method (hexokinase) and successfully applied to the determination of glucose in human serum.     

Novel glucose biosensor based on a glassy carbon electrode modified with hollow gold nanoparticles and glucose oxidase

A novel glucose biosensor is presented as that based on a glassy carbon electrode modified with hollow gold nanoparticles (HGNs) and glucose oxidase. The sensor exhibits a better differential pulse voltammetric response towards glucose than the one based on conventional gold nanoparticles of the same size. This is attributed to the good biological conductivity and biocompatibility of HGNs. Under the optimal conditions, the sensor displays a linear range from 2.0?×?10^?6 to 4.6?×?10^?5?M of glucose, with a detection limit of 1.6?×?10^?6?M (S/N?=?3). Good reproducibility, stability and no interference make this biosensor applicable to the determination of glucose in samples such as sports drinks.

Sensitive spectrophotometric detection of dopamine,levodopa and adrenaline using surface plasmon resonance band of silver nanoparticles

A simple and effective procedure is proposed for spectrophotometric determination of catecholamines; Dopamine (1), L-Dopa (2) and Adrenaline (3). It was found that the reduction of Ag⁺ to silver nanoparticles (Ag-NPs) by these catecholamines in the presence of polyvinylpyrrolidone (PVP) as a stabilizing agent produced very intense surface plasmon resonance peak of Ag-NPs. The plasmon absorbance of the Ag-NPs allows the quantitative spectrophotometric detection of the catecholamines. The calibration curves derived from the changes in absorbance at λ = 440 nm were linear with concentration of Dopamine, Levodopa and Adrenaline in the range of 3.2×10^?6? 2.0×10^?5 M, 1.6×10^?7 ? 1.0×10^?5 M, 1.5×10^?6? 4.0×10^?5 M, respectively. The detection limits (3σ) were 1.2×10^?6 M, 8.6 ×10^?8 M, 9.7 ×10^?7 M for the Dopamine, L-Dopa and Adrenaline, respectively. The method was applied successfully to the determination of catecholamines in Ringer’s injection serum.     

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.     

Magnetite NPs@C with Highly‐Efficient Peroxidase‐Like Catalytic Activity as an Improved Biosensing Strategy for Selective Glucose Detection

This work reports the novel application of carbon‐coated magnetite nanoparticles (mNPs@C) as catalytic nanomaterial included in a composite electrode material (mNPs@C/CPE) taking advantages of their intrinsic peroxidase‐like activity. The nanostructured electrochemical transducer reveals an enhancement of the charge transfer for redox processes involving hydrogen peroxide. Likewise, mNPs@C/CPE demonstrated to be highly selective even at elevated concentrations of ascorbic acid and uric acid, the usual interferents of blood glucose analysis. Upon these remarkable results, the composite matrix was further modified by the addition of glucose oxidase as biocatalyst, in order to obtain a biosensing strategy (GOx/mNPs@C/CPE) with enhanced properties for the electrochemical detection of glucose. GOx/mNPs@C/CPE exhibit a linear range up to 7.5×10^?3 mol L^?1 glucose, comprising the entirely physiological range and incipient pathological values. The average sensitivity obtained at ?0.100 V was (1.62±0.05)×10⁵ nA L mol^?1 (R²=0.9992), the detection limit was 2.0×10^?6 M while the quantification limit was 6.1×10^?6 mol L^?1. The nanostructured biosensor demonstrated to have an excellent performance for glucose detection in human blood serum even for pathological values.     

Electrochemiluminescence Biosensor for Glucose Based on Graphene/Nafion/GOD Film Modified Glassy Carbon Electrode

Glucose oxidase(GOD) was encapsulated in the Graphene/Nafion film modified glassy carbon electrode(GCE) and used as an ECL sensor for glucose. The GOD retains its bioactivity after being immobilized into the composite film. The sensor gives a linear response for glucose in the range of 2.0×10^?6–1.0×10^?4 mol/L with a detection limit of 1.0×10^?6 mol/L. The sensor showed good stability, the RSD for continuous scanning for 5.0×10^?5 mol/L glucose was 4.21 % (n=5). After being stored in 0.05 mol/L pH 7.4 PBS in 4 °C for two weeks, the modified electrode maintains 80 % of its initial activity. The glucose sensor provides new opportunity for clinical diagnosis applications.     

The study of synergistic effects of ZnO decorated graphene nanosheets and room temperature ionic liquid for analysis of raloxifene in pharmaceutical samples

Raloxifene is an important estrogen receptor modulator with many side effects, and determination of this drug is very important in biological samples. The present research describes a ZnO decorated graphene nanosheet (ZnO/GrNS)/ionic liquid based electrochemical sensor for the measurement of raloxifene. The ZnO/GrNS were synthesized via direct chemical precipitation process and characterized using the SEM-EDAX technique. Due to excellent conductivity of ZnO/GrNS and ionic liquid, the suggested electrochemical sensor exhibited improved electrochemical response for raloxifene. After optimization of electrochemical conditions and at the best state, the fabricated electrode displayed two linear dynamic ranges (1.0?×?10^?10–5.0?×?10^?6 and 1.0?×?10^?6–5.0?×?10^?4 M) with a detection limit (DL) of 0.07 nM. Quantification analysis of raloxifene was successfully evaluated using the suggested sensor in pharmaceutical samples.     

Pt nanoparticles modified Au nanowire array for amperometric and potentiometric detection of glucose

A new glucose biosensor, based on the modification of highly ordered Au nanowire arrays (ANs) with Pt nanoparticles (PtNPs) and subsequent surface adsorption of glucose oxidase (GOx), is described. Morphologies of ANs and ANs/PtNPs were observed by scanning electron microscope. The electrochemical properties of ANs, ANs/GOx, ANs/PtNPs, and ANs/PtNPs/GOx electrodes were compared by cyclic voltammetry. Results obtained from comparison of the cyclic voltammograms show that PtNPs modification enhances electrochemical catalytic activity of ANs to H₂O₂. Hence, ANs/PtNPs/GOx biosensor exhibits much better sensing to glucose than ANs/GOx. Optimum deposition time of ANs/PtNPs/GOx biosensor for both amperometric and potentiometric detection of glucose was achieved to be 150 s at deposition current of 1?×?10^?6 A. A sensitivity of 0.365 μA/mM with a linear range from 0.1 to 7 mM was achieved for amperometric detection; while for potentiometric detection the sensitivity is 33.4 mV/decade with a linear range from 0.1 to 7 mM.     

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。     

Pulsed coulometric detection of carbohydrates at a constant detection potential at gold electrodes in alkaline media

A significant increase in the signal-to-noise ratio for the pulsed amperometric detection (PAD) of carbohydrates at gold electrodes is obtained by increasing the length of the current integration period (t_i) from the traditional value of 16.7 ms (i.e., $\text{1}\text{60}$ Hz). For t_i > 16.7 ms, the integrated response (q, coulombs) is plotted as the signal. This pulsed coulometric detection (PCD) is applied in a flow-injection system. For t_i = 500 ms, the detection limit with the instrumentation used is 1 μM (S/N = 2) for glucose which is a significant improvement on the value 35 μM found with PAD. The absolute detection limits for glucose and sucrose are ca. 50 pmol and 125 pmol, respectively, in 50-μl samples. Calibration plots (q_p vs. C^b) for PCD are linear over significantly larger dynamic ranges than those observed for PAD because of the lower detection limits.     

Flow-injection determination of paraoxon by inhibition of immobilized acetylcholinesterase

Two flow-injection methods (continuous-flow and stopped-flow) are proposed for the determination of paraoxon, applying the dual-injection technique and spectrophotometric detection. They are based on the inhibition of the acetylcholinesterase-catalysed hydrolysis of α-naphthyl acetate and subsequent reaction of the α-naphthol produced with p-nitrobenzenediazonium fluoroborate. For the continuous-flow system the calibration graph was linear from 5 × 10^?7 to 1.5 × 10^?5 M, the relative standard deviation (r.s.d.) (n=6) for an 8 × 10^?6 M standard was 1.4%, the limit of detection (3σ) was 4 × 10^?7 M and the sample throughput was ca. 60 h^?1. For the stopped-flow system the linear range was from 1 × 10^?8 to 4 × 10^?7 M, the r.s.d. for a 2.5 × 10^?7 M standard was 0.9%, the limit of detection was 8 × 10^?9 M and the sample throughput was 30 h^?1.     

Electro‐oxidation and Determination of Tripelennamine Hydrochloride at MWCNT‐CTAB Modified Glassy Carbon Electrode

An electrochemical method for the determination of tripelennamine hydrochloride (TPA) using cetyltrimethylammoniumbromide‐multiwalled carbon nanotubes modified glassy carbon electrode (MWCNT‐CTAB/GCE) was developed. Because of good electrical conductivity of MWCNT and catalytic behavior of CTAB, new electrode significantly enhances the sensitivity for the detection of TPA. Parameters such as amount of modifier suspension, scan rate, pH of measure solution, heterogeneous rate constant were investigated. The electrode exhibits a linear potential response in the range of 1.0×10^?8 M to 3.0×10^?6 M with a detection limit of 2.38× 10^?9 M. The modified electrode was successfully applied to the determination of TPA in pharmaceutical and real samples.     

Spectrophotometric Determination of Hydrogen Peroxide and Glucose Based on Hemin Peroxidase-Like Catalyzed Oxidation of Bromopyrogallol Red

In an ammonium buffer medium at pH 8.9–9.5, hemin exhibits mimetic peroxidase activity, and has a catalytic effect on the oxidative decoloration of bromopyrogallol red (BPR) with hydrogen peroxide. On this basis and in presence of ethanol as an effect-enhancing agent, a spectrophotometric determination of hydrogen peroxide is described with an apparent molar absorptivity of 4.00×10⁴?l?mol^?1?cm^?1 and a linear range from 3.2×10^?7 to 3.2×10^?5?mol?l^?1. BPR has advantages over some of widely used chromogenic substrates in aspects of sensitivity, simplicity and detection wavelength, while hemin has better stability than peroxidase. The system can be easily coupled with a glucose oxidase-catalyzed reaction, and glucose in the concentration range of 6.0×10^?7? 3.2×10^?5?mol?l^?1 is spectrophotometrically determined. The method has been applied to the analyses of synthetic water and human serum samples. The Michaelis parameters and the mechanism of the mimetic peroxidase reaction are also investigated.     

A Bipotentiostat Based 4‐Electrode Detection System for HPLC Analysis

With the assist of a microcomputer interfacing, a bipotentiostat in corporated 4‐electrode detection system was developed as a versatile electrochemical detector for HPLC. An amperometric chromatogram and two three‐dimensional chromatovoltammograms characterizing the electrochemical characteristics of analytes can be obtained in a single chromatographic run. By following the three operation modes developed, both the oxidizable and reducible analytes contained in sample solutions can be determined. The analytical capability of the 4‐electrode detection system was demonstrated by the analysis of solutions containing hydroquinone, catechol and ascorbic acid. From the calibration graphs obtained, linear coefficients better than 0.9992 were found for hydroquinone and catechol in a concentration range of 1.0 × 10^?4 to 1.0 × 10^?7 M, and a linear coefficient of 0.9929 was found for ascorbic acid in a concentration range of 1.0 × 10^?4 to 1.0 × 10^?6 M. The detection limits (based on S/N = 3) found were about 1.0 × 10^?7 M for hydroquinone and catechol and was 1.0 × 10^?6 M for ascorbic acid.     

Electrochemiluminescent Detection Method for Glyphosate in Soybean on Carbon Fiber-ionic Liquid Paste Electrode

A carbon fiber paste electrode using ionic liquid as the binder (CFILE) was fabricated. The electrochemical characteristics of the electrode was examined in ferro‐/ferricyanide solution and showed better conductivity and reversibility when compared with graphite paste‐ionic liquid electrode (GPILE) and a little better than that on the carbon nanotube paste‐ionic liquid electrode (CNTILE). Glyphosate (GLY), a pesticide, exhibited excellent catalysis to the oxidation of Ru(bpy)²⁺₃ on CFILE and brought an obvious enhancement to the electrochemiluminescence (ECL) intensity of Ru(bpy)²⁺₃. Based on the catalytic ability of GLY, a simple ECL method for GLY detection had been established. Under optimum conditions, the enhanced ECL intensities were found to had linearly respond to the GLY concentration between 3.0×10^?7 and 3.0×10^?5 mol/L, and the detection limit (S/N=3) was 2.0×10^?7 mol/L. The electrode also showed excellent sensitivity in detecting GLY‐spiked soybean samples. The linear range for GLY in soybean samples was 1.0×10^?6–4.0×10^?5 mol/L and the detection limit was 5.0×10^?7 mol/L, equal to 8.45 µg GLY in per gram of soybean. The detection limit in soybean sample was lower than the USA, EU regulation and so on. If the method is coupled with the separation technology, it can be applied to detect the GLY in the contaminated samples.     

A sensitive electrochemical sensor for detection of rutin based on a gold nanocage‐modified electrode

In this article, an electrochemical sensor based on a gold nanocage (AuNC)‐modified carbon ionic liquid electrode (CILE) was fabricated and applied to the sensitive rutin determination. The presence of AuNCs on the electrode surface greatly improved the electrochemical performance of the working electrode due to its specific microstructure and high metal conductivity. Electrochemical behavior of rutin on AuNCs/CILE was studied using cyclic voltammetry and differential pulse voltammetry with the related electrochemical parameters calculated. Under the optimal experimental conditions, the oxidation peak current of rutin and its concentration had good linear relationship in the range from 4.0 × 10^?9 to 7.0 × 10^?4 mol/L with a low detection limit of 1.33 × 10^?9 mol/L (3σ). This fabricated AuNCs/CILE was applied to direct detection of the rutin concentration in drug samples with satisfactory results, showing the real application of AuNCs in the field of chemically modified electrodes.     

Quantitative Analysis of Prometrine Herbicide by Liquid–Liquid Extraction Procedures Coupled to Electrochemical Measurements

A sensitive method is proposed for the preconcentration and quantification of the herbicide Prometrine (PROM) at a liquid‐liquid interface employing square‐wave voltammetry. The preconcentration stage was based on liquid‐liquid extraction methodology and the PROM quantification was carried out from the peak current of square‐wave voltammograms. Under the experimental conditions employed, linear calibration curves in the concentration range 1.0×10^?6 M–5.0×10^?5 M, with detection limit equal to 1.5×10^?6 M were obtained without pretreatment of the samples. This linear range, as well as detection limit could be extended towards lower concentrations when a pretreatment procedure was employed. In this way, linearity of calibration curves between 8.0×10^?8 M and 2.4×10^?7 M and detection limit of 1.0×10^?7 M, were observed. On the other hand, the standard addition method was also used as an alternative and an appropriated quantification technique for this system. A linear concentration range between 1.0×10^?6 M and 2.7×10^?5 M, with a correlation coefficient of 0.997, was obtained. This procedure has also a promising application in the separation of herbicides from other interferents, present in real samples, previous to their quantification.     

Determination of microgram amounts of carbon in the for of carbamate by non-aqueous electrolytic conductivity detection

An absorption/detection system is described for the determination of carbon at and below microgram detection level. The carbon dioxide formed by combustion of an organic substances (solid or in solution) is led into a simple absorption/detection system containing 2.00 cm³ of an ethanolic 2 M solution of 3-methoxypropylamine. The conductivity of the carbamate solution formed is measured by means of platinum electrodes built in the absorption tube, and the integrated d.c. voltage signal obtained is fed to a precision digital voltmeter. Detector response is linear up to 6.6 μg of carbon, and the detection limit is 2 × 10^?2 μg. A single determination takes 5 min. Precision was found to be better than +? 1.0% (P-=95%) for 1–6 μg or carbon.     

Electrochemical investigation and determination of ceftazidime in pharmaceutical dosage forms and human urine

A voltammetric study of the oxidation of Ceftazidime (CEFT) has been carried out at the glassy carbon electrode by cyclic, differential pulse (DPV) and square wave (SWV) voltammetry. The oxidation of CEFT was irreversible and exhibited diffusion controlled process depending on pH. The oxidation mechanism was proposed and discussed. According to the linear relationship between the peak current and concentration, DPV and SWV voltammetric methods for CEFT assay in pharmaceutical dosage forms and human urine were developed. For analytical purposes, a well resolved diffusion controlled voltammetric peak was obtained in 0.1 M H₂SO₄ at 1.00 and 1.02 V for differential pulse and square wave voltammetric techniques, respectively. The linear response was obtained within the range of 4 × 10^?6?8 × 10^?5 M with a detection limit of 6 × 10^?7 M for differential pulse and 4 × 10^?6–2 × 10^?4 M with a detection limit of 1 × 10^?6 M for square wave voltammetric technique. The determination of CEFT in 0.1 M H₂SO₄ was possible over the 2 × 10^?6–1 × 10^?4 M range in urine sample for both techniques. The standard addition method was used for the recovery studies.     

Determination of chlorite at very low levels by using differential pulse polarography

A method is reported for the determination of μgl^?1 levels of chlorite by using differential pulse polarography. The electrochemical reduction of chlorite was studied between pH 3.7 and 14 and in an ionic strength range of 0.05–3.0 M. The optimum conditions are pH 4.1–4.4 and an ionic strength of 0.45 M. The current under these conditions is diffusion-controlled and is a linear function of chlorite concentration ranging from 2.77×10^?7 to 2.80×10^?4 M (19 μgl^?1 to 19 mg l^?1). The imprecision is better than ±1.0% and ±3.4% at concentrations of 2.87×10^?5 M and 1.74×10^?6M, respectively, with a detection limit of 1×10^?7 M (7μgl^?1). An interference study and the application of this method for determining chlorite in drinking water are reported.