NADH Electrocatalytic Oxidation on Gold Nanoparticle‐Modified PVC/TTF‐TCNQ Composite Electrode. Application as Amperometric Sensor

We herein report on the electrocatalytic activity towards the oxidation of NADH of a PVC/TTF‐TCNQ composite electrode modified with gold nanoparticles. This electrocatalytic property allows proposing this system as a new alternative for amperometric determination of NADH, without need to add another mediator. The sensor shows a linear response to NADH over a concentration range from 5.0×10^?6 M up to 5.0×10^?4 M, with a sensitivity of 11.22±0.5 mA M^?1 and a detection limit (S/N=3) of 4.0×10^?6 M for measurements in batch and similar data in FIA.     

Cyclic voltammetry of Tifluadom at a C18-modified carbon-paste electrode

Tifluadom, N-[5-(2-fluorophenyl)-2,3-dihydro-methyl-1H-1,4-benzodiazepine]-2-4-methyl-3-thiophene carboxamide, was determined by using a carbon-paste electrode modified with C₁₈ μBondapak. Adsorption on the electrode served as a preconcentration step which improved the limit of detection. Preconcentration for 5 min (open circuit) gave a linear range of 2.2×10^?7 M?4.5×10^?6 M with a detection limit of 1.3×10^?7 M (%C₁₈=25, w/w) for Tifluadom in Britton-Robinson buffer pH 6. The determination of Tifluadom added to urine required no preliminary treatment; the detection limit was 1.3×10^?6 M.     

Fluorescence quenching of thionine by reduced nicotinamide adenine dinucleotide

Reduced nicotinamide adenine dinucleotide (NADH) is shown to quench the fluorescence of thionine. Quenching of thionine is extremely efficient with a half quenching concentration of only 16.1 × 10⁻⁶ M NADH. A Stern—Volmer plot is linear over the NADH concentration range from 1 to 20μM. The corresponding Stern—Volmer quenching constant is 6.2 × 10⁴ M⁻¹ and the limit of detection for NADH measurements is 1.6 × 10⁻⁶ M. Process of quenching is attributed to the formation of an exciplex between thionine and NADH. Potential analytical features of this system are discussed.     

Consecutive determination of rutin and quercetin by spectrophotometric measurements

The consecutive determination of rutin and quercetin without any pretreatment for separation was examined in methanol solutions by a conventional and a two-wavelength spectrophotometry. Based the tendency of quercetin to form more stable metal complexes compared to rutin, quercetin can be determined through the tin(II) complex formation without interference from rutin. The method was applied to the determination of quercetin in the concentration range of 3.0 × 10^?6 to 2.0 × 10^?5M.Quercetin is apt to be oxidized by oxygen rather than rutin, especially in the presence of copper(II), whereas rutin is not decomposed under such a condition. After removal of quercetin through copper(II)-catalyzed oxidation, rutin ranging in concentration from 2.0 × 10^?6 to 2.0 × 10^?M was determined by the absorbance measurement of rutin-copper(II) complex in slightly alkaline methanol media.Both rutin and quercetin were determined directly by two-wavelength spectrophotometry, without adding any complex forming metals; the lower limit of detection was about 1.0 × 10^?5M. The method was extended to the determination of a smaller amounts of rutin and quercetin using the absorption peaks of their zirconium(IV) complexes, and the determination of both components in the range of 5.0 × 10^?6 to 3.0 × 10^?5M was made with a relative error of within ±4%.     

Flow-injection determination of d-mannitol with immobilized mannitol dehydrogenase

A flow-injection system is described for the determination of d-mannitol. Mannitol dehydrogenase is immobilized on poly(vinyl alcohol) beads and packed in a column (5 cm × 4 mm i.d.). The NADH formed is detected fluorimetrically. The response is linear between 5 × 10^?7 and 1 × 10^?4 M mannitol and the detection limit is 1 × 10^?7 M. The throughput is 30 samples per hour. The reactor is stable for at least 8 weeks.     

Properties of bacterial luciferase/NADH : FMN oxidoreductase and firefly luciferase immobilized onto sepharose

NADH : FMN oxidoreductase and bacterial luciferase have been efficiently coimmobilized onto Sepharose 4B. This luminescent immobilized enzyme system can be used to assay NADH. The assay is rapid and sensitive with a lower limit of detection of 0.2 pmol/assay tube. The intra-assay precision was 3.5% at 2 × 10^-5 M and 5.8% at 2 × 10^-6 M NADH. Light intensity was proportional to NADH concentration from 0.2 to 1000 pmol. Added serum and certain dehydrogenases were found to be inhibitory; however, inhibition could be eliminated by a combination of heat treatment and dilution. Firefly luciferase has also been immobilized onto both Sepharose 4B and CL 6B. The detection limit for ATP using this immobilized enzyme was 0.2 pmol and the assay was linear from 0.2 to 2000 pmol. The intra-assay precision was 4.8% at 2 × 10^-4 M and 3.2% at 1 × 10^-5 M ATP. The immobilized enzymes remained fully active when rapidly frozen in the presence of glycerol and DTT. Such preparations could be stored for at least two months with no loss of activity. A variety of different compounds were used to block any remaining reactive groups on the Sepharose following immobilization of the enzymes. Glycine, 2-aminoethanol, and ethylenediamine were examined. The preparations where ethylenediamine was used as a blocking agent exhibited better activity and stability than the others.     

Electrophoretic determination of 1-methyl-2-mercaptoimidazole in the pharmaceutical preparation mercazolyl

The conditions for the quantitative determination of 1-methylimidazoline-2-thione with the use of a Kapel’ 103-R capillary electrophoresis system were optimized (acetate buffer; pH 4.5; U = 20 kV). The analytical range of the procedure is 1.5 × 10^?4?1.8 × 10^?3 M (the limit of detection is 4.6 × 10^?5 M; RSD = 2.5%). The tablets of Mercazolyl from Akrikhin (Moscow) and Zdorov’e (Kharkov) were analyzed.     

Determination of Tetracycline by Microdroplet Hydrodynamic Adsorptive Voltammetry Using a Multiwalled Carbon Nanotube Paste Rotating Disk Electrode

A novel and simple method is proposed for the determination of tetracycline by adsorptive voltammetry in a droplet using a carbon nanotube paste rotating disk electrode (CNTP-RDE). An enhanced electrochemical oxidation response of tetracycline was observed in pH 8.2 supporting electrolyte by the addition of a long-chain cationic surfactant, such as benzyldimethyltetradecylammonium chloride (zephiramine). Under the optimized experimental conditions, the calibration curve was linear across a tetracycline concentration range from 1.0?×?10^?7 to 2.0?×?10^?6 M. The limit of detection and sensitivity were 4.0?×?10^?8 M and 0.9358?A M^?1, respectively. This method was successfully employed for the determination of tetracycline in milk samples.     

A kinetic determination of ultramicroquantities of some biologically active substances

A new kinetic method for the determination of ultramicroquantities of adrenaline, noradrenaline, thyroxine, and 5-hydroxytryptophan is presented. The method is based on the effect of these organic substances on the oxidation of pyrocatechol violet with hydrogen peroxide, catalyzed by Cu(II) ions.In order to find out the experimental conditions under which this effect is optimum, the kinetics of the above-mentioned indicator reaction in the presence of the compounds to be determined was studied in detail.Adrenaline and noradrenaline were determined at concentrations ranging from 2.0 × 10^?6 to 8.0 × 10^?6M, thyroxine at concentrations varying from 1.0 × 10^?6 to 10.0 × 10^?6M, and 5-hydroxytryptophan over the concentration range 7.7 × 10^?7–32.0 × 10^?7M. In these determinations the standard deviation was lower than 10%.     

Determination of tetracycline by flow injection with chemiluminescence detection

Tetracycline hydrochloride (4 × 10^?5?1 × 10^?3M) in a 40-μl aqueous sample is determined in a flow system by measurement of the chemiluminescence emitted on reaction with bromine (9.3 × 10^?3 M) at pH 10.4 (carbonate buffer). The limit of detection is 1.6 nmol per 40-μl injection.     

Methylated Azopyridine as a New Electron Transfer Mediator for the Electrocatalytic Oxidation of NADH

Carbon ionic liquid electrode (CILE) has been modified with a new synthesized mediator i.e. N,N′‐dimethyl‐4,4′‐azopyridinium hexafluorophosphate (MAZPHP) via sol process and the electron transfer mediating characteristics of this mediator has been evaluated. 4,4′‐Azopyridine (AZP) did not show any electrocatalytic activity toward the selected probe, NADH, while its synthesized methylated derivative, MAZPHP, is a very efficient mediator for the electrocatalytic NADH oxidation. Cyclic voltammetry of MAZPHP/Sol/CILE exhibited a pair of reversible peaks corresponding to incorporated mediator with a formal potential of about 221 mV vs. Ag/AgCl. MAZPHP/Sol/CILE is free from fouling effects by the oxidation products of NADH which generally give hindrance to amperometric detection of NADH. Using amperometric technique, NADH can be determined in the range of 1.0×10^?5 M to 1.4×10^?3 M with a detection limit of 2.0×10^?6 M.     

Study of Electrooxidation Behavior of Nitrite on Gold Nanoparticles/Graphitizing Carbon Felt Electrode and Its Analytical Application

In this work, a gold nanoparticles/graphitizing carbon felt electrode (AuNPs/GCFE) was fabricated and a disposable sensor was thus fabricated to detect nitrite quickly and conveniently. The kinetic parameters of the electrode were studied in phosphate buffer solution (PBS). Under the optimal conditions, by using cyclic voltammetry, the oxidation peak current was linear with the concentration of nitrite in the range from 1.00 × 10^?6 M to 3.35 × 10^?3 M, with a detection limit of 9.50 × 10^?7 M (3S/k). The influence of various anions on nitrite detection was studied, and the results showed that the fabricated sensor had good specificity toward nitrite.     

Electrochemical Study of Interaction Between Clozapine and DNA and Its Analytical Application

Abstract

The interaction between clozapine (CLZ) as an orally administrated antipsychotic drug with double stranded calf thymus DNA (dsDNA) was investigated at electrode surface using differential pulse voltammetry (DPV). Activated carbon paste electrode (CPE) was modified with dsDNA and used for monitoring the changes of the characteristics peak of CLZ in 0.05 M acetate buffer (pH 4.3). The adsorptive stripping voltammetry on dsDNA‐modified carbon paste electrode (dsDNA‐CPE) was used for determination of very low concentration of CLZ. Under optimal conditions, the oxidation peak current is proportional to CLZ concentration in the range of 7×10^?9?1.2×10^?6 mol l^?1 with a detection limit of 1.5×10^?9 mol l^?1 for 180 s accumulation time by DPV. The proposed dsDNA‐CPE was successfully used for determination of CLZ in human serum samples with recovery of 97.0±2.5%.     

Sensitive voltammetric assay of etoposide using modified glassy carbon electrode with a dispersion of multi-walled carbon nanotube

A sensitive electroanalytical method for the determination of anticancer drug etoposide (ETP) using adsorptive stripping differential pulse voltammetry (AdSDPV) at a multi-walled carbon nanotube-modified glassy carbon electrode (MWCNT-modified GCE) is presented. The surface morphology of modified electrode was characterized by scanning electron microscopy. The effects of accumulation time and potential, pH, scan rate, and amount of MWCNT suspension were investigated. The calibration curve was linear in the concentration range of 2.0?×?10^?8–2.0?×?10^?6 M with the detection limit of 5.4?×?10^?9 M. The reproducibility of the peak current was found at 1.55 % (n?=?5) RSD value in pH 6.0 Britton–Robinson buffer for the MWCNT-modified GCE. The method was then successfully utilized for the determination of ETP in pharmaceutical dosage form, and a recovery of 99.55 % was obtained. The possible oxidation mechanism of ETP was also discussed. The proposed electroanalytical method using MWCNT-modified GCE is the most sensitive method for the determination of ETP with lowest limit of detection in the previously published electrochemical methods.     

RP-LC Determination of Residual Monomers in Polycarboxylate Superplasticizers

A procedure was developed for the determination of residual monomers in polycarboxylate superplasticizer by reversed-phase high performance liquid chromatography. Seven kinds of residual monomers were quantitatively determined on a SinoChrom ODS-BP (C18) column and UV detector at 205 nm. The mobile phases which were used to determine micromolecular monomers were composed of acetonitrile and phosphate buffer solution (0.05 mol L^?1, pH = 3) in the ratio of 8:92 (v/v). While the mobile phases for long side-chain monomers testing were composed of acetonitrile and phosphate buffer solution (0.05 mol L^?1, pH = 6.5) in the ratio of 40:60 (v/v). The linear response ranged from 4.0 × 10^?6?C2.0 × 10^?3 mol L^?1. The detection limit was 0.12 × 10^?5?C0.8 × 10^?5 mol L^?1. Determination of real samples showed that relative standard deviation of high conversion rate samples was 3.1?C8.7% and standard addition recovery ratio was 91.5?C102.8%. While the relative standard deviation of low conversion rate samples was less than or close to 1% and the standard addition recovery ratio was 96.3?C103.1%.     

Determination of ferulic acid in Chinese proprietary medicine based on a poly-glutamic acid film sensor

The poly-glutamic acid modified electrode has been prepared by direct electro-polymerization of D-glutamic acid on the surface of glassy carbon electrode. In pH 4.2, 0.1 mol L^?1 HAc-NaAc buffer solution, the film modified electrode exhibited remarkable enhancement effect to the electrochemical responses of ferulic acid. The action mechanism was preliminarily explored. In the range of 2.0 × 10^?7 to 1.0 × 10^?5 mol L^?1, and 1.0 × 10^?5 to 3.0 × 10^?4 mol L^?1, the oxidation peak current has a linear relationship to the concentration, and the detection limit was estimated to be 7.0 × 10^?8 mol L^?1. This method has been adopted to detect trace amount of ferulic acid in Chinese proprietary medicine, and the recovery was from 97.8 to 102.4%.     

Electrocatalytic Oxidation of Hydrazine at the Poly(Glutamic Acid) Chemically Modified Electrode and Its Amperometric Determination

ABSTRACT

The electrochemical polymerization of glutamic acid at the glassy carbon electrode was investigated in phosphate buffer solution by cyclic voltammetry. The applied voltage range, pH of electrolyte, cyclic number were explored for optimal polymerization conditions. The resulting film exhibits an electrocatalytic ability to hydrazine, reducing the overpotential by 500mV. The electrocatalytic response of hydrazine is evaluated with regard to pH, scan rate, applied voltage, hydrazine concentration and other variables. The rate constant of the catalytic reaction was 1.2 × 10⁴ M^?1.s^?1. When used as amperometric detector, the modified electrode yields a detection limit of 1 × 10^?8 M hydrazine. The electrode is rather stable even after use for a month and a reproducible response was obtained.     

Sol‐Gel‐Derived Biosensor Based on Plant Tissue: The Inhibitory Effect of Atrazine on Polyphenol Oxidase Activity for Determination of Atrazine

This work presents a sol‐gel based biosensor for atrazine determination which has been obtained by introducing the enzyme polyphenol oxidase from apple tissue in a sol‐gel matrix. Apple tissue acts as a molecular recognition element. Atrazine is an inactive compound electrochemically; redox coupling of dopamine was used for studying atrazine behavior. Atrazine was determined by monitoring the inhibition power of polyphenol oxidase activity. The measurements were performed in 0.1 M KH₂PO₄‐NaOH buffer (pH 7.5). The effect of various experimental parameters such as pH, concentration of buffer, concentration of dopamine, incubation time and matrix composition has been investigated for optimum analytical performance. The biosensor consisted of 10.3% (w/w) of apple tissue. The bioelectrode exhibits a linear response for dopamine and atrazine concentrations in the range of 5.66 × 10^?6?2.27 × 10^?3M and 1 × 10^?5 ?1 × 10^?4 M with a detection limit of 4.2 × 10^?6 and 5.5 × 10^?6 M, respectively. A correlation coefficient of 0.9945 and a relative standard deviation (R.S.D.) of 3.29% for dopamine, 0.9944 and 3.69% for a trazine were achieved.     

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.     

Enhancement effect of cysteine on anodic stripping voltammetry of copper

The anodic stripping behaviour of copper in the presence of compounds with a mercapto group, such as cysteine, was investigated. In the presence of cysteine, a copper stripping wave at ?0.12 V vs. SCE decreased, and instead a new sharp wave was observed at more positive potential. Its peak height increased with increasing concentration of cysteine, and at 1 × 10^?5M cysteine it became about seven times as large as that observed in the absence of cysteine. Then the method using this enhanced wave was studied for the determination of trace cupric ion. The results were that the relative standard deviation for five repetitive determinations was about 4% at 10^?8M Cu(II) and the detection limit was 6 × 10^?10M Cu(II). From the investigation by means of cyclic voltammetry, it was found that this enhanced wave was due to the transformation from a cupric—cysteinate complex to a mercuric—cysteinate complex.