Determination of Uric Acid in Human Urine by Ion‐exclusion Chromatography with UV Detection Using Pure Water as Mobile Phase

A simple, rapid and accurate ion‐exclusion chromatographic method coupled with a UV detector for the determination of uric acid in human urine samples has been developed. The separation was carried out on an ion‐exclusion column using only pure water as mobile phase. The detection wavelength was 254 nm and urine sample was injected directly without any pretreatment. Furthermore, the retention behavior of uric acid on the ion‐exclusion column was researched when pure water and 1 mmol·L^?1 HCl were used as mobile phase, respectively. The stability of uric acid was also further investigated within 28 days. In this method, the linear range of the calibration curve for uric acid was 0.25–100 mg·L^?1, and the detection limit calculated at S/N=3 was 0.02 mg·L^?1. The proposed ion‐exclusion chromatographic method has been used for the determination of uric acid in human urine.     

Simultaneous Determination of Dopamine and Uric Acid by Electrocatalytic Oxidation on a Carbon Paste Electrode Using Pyrogallol Red as a Mediator

A sensitive and selective electrochemical method for the simultaneous determination of dopamine (DA) and uric acid (UA) was developed using a pyrogallol red modified carbon paste electrode. Under the optimized conditions, the peak current was linearly dependent on 1.0–700.0 μmol L^?1 DA and 50.0–1000.0 μmol L^?1 UA. The detection limits for DA and UA were 0.78 μmol L^?1 and 35 μmol L^?1, respectively. Finally, this method was also examined for the determination of DA and uric acid in real samples such as drugs and urine.     

Application of simultaneous separation and derivatization for the determination of α‐lipoic acid in urine samples by high‐performance liquid chromatography with spectrofluorimetric detection

To help to clarify therapeutic functions of lipoic acid (LA) in biochemical and clinical practice we have elaborated a fast, simple and accurate HPLC method enabling determination of LA in human urine. The proposed analytical approach includes reduction of LA with tris(2‐carboxyethyl)phosphine and simultaneous separation and derivatization of the analyte with butylamine and o‐phthaldialdehyde followed by spectrofluorimetric detection at λ_ex = 340 nm and λ_em = 440 nm. The assay was performed using gradient elution and the mobile phase containing 0.0025 mol L^?1 o‐phthaldialdehyde in 0.0025 mol L^?1 NaOH and acetonitrile. Linearity of the detector response for LA was observed in the range of 0.3–8 μmol L^?1. Limits of detection and quantification for LA in urine samples were 0.02 and 0.03 μmol L^?1, respectively. The total analysis time, including sample work‐up, was <20 min. The analytical procedure was successfully applied to analysis of real urine samples delivered from six healthy volunteers who received a single 100 mg dose of LA.     

Studies on reaction of reduced lipoic acid with Mukaiyama reagent and its application for pharmaceutical and food analysis

A new sensitive method for the determination of lipoic acid (LA) in selected food items based on its reaction with Mukaiyama reagent (2-chloro-1-methylpyridinium iodide, CMPI) was developed. It was stated that CMPI reacts with reduced form of lipoic acid (dihydrolipoic acid, DHLA) and the stable product is produced. The spectrum of the labeled form of DHLA exhibits new band at 312?nm. Based on its spectral characteristics new spectrophotometric and UV–high-performance liquid chromatography (HPLC) methods of LA determination were elaborated. Both methods allowed determination of the analyte in the concentration range of 5?×?10^?6–1?×?10^?4?mol?L^?1 with limit of detection 0.39?×?10^?6 and 0.77?×?10^?6?mol?L^?1 for spectrophotometric and HPLC method, respectively. The practical usability of newly developed methods was checked by determination of lipoic acid contents in its pharmaceutical preparate Revitanerw. The proposed method was precise and accurate. The relative error of determination did not exceed ±0.067%. As chromatographic method allowed the determination of analyte in the presence of complex matrix, it was applied for assay of free fraction of α-lipoic acid in selected food items. A procedure of LA isolation from biological matrix was developed. The extraction with dichloromethane allowed quantitative recovery at 102.94?±?4.20%. The green barley appeared to be the richest source of LA.     

Determination of atorvastatin in human plasma by magnetic solid-phase extraction combined with HPLC and application to a pharmacokinetic study

A simple and sensitive analytical procedure by solid-phase extraction method combined with high-performance liquid chromatography and using of graphene–magnetite nanomaterials as sorbent has been developed for the determination of atorvastatin in human plasma. A magnetic solid-phase extraction method as a simple, fast, and efficient extraction technique has been used for sample preparation. A solid nanocomposite material, graphene nanosheets decorated with magnetite nanoparticles, was used as a magnetic adsorbent and the adsorption process was optimized in this study. RP C18 column was used with mobile phase composed of acetonitrile–10?mM orthophosphoric acid by isocratic elution with the flow rate of 1?mL?min^?1. Fluorimetric detection was used by the excitation wavelength at 282?nm and the emission wavelength at 400?nm. It was found that the calibration curve was linear in the 30–150?ng?mL^?1. Limit of detection and limit of quantitation values were found to be 10 and 30?ng?mL^?1, respectively. The intra-day and inter-day relative standard deviation values were less than 5.27%. It has been concluded that the new developed method provides fast, simple, cost reduced, and sensitive assay for atorvastatin determination in human plasma. This method is also applied to a pharmacokinetic study.     

Spectrophotometric determination of Chromium(VI) using cyclam as a reagent

A simple, rapid, sensitive, and inexpensive method for spectrophotometric determination of chromium(VI), based on the absorbance of its complex with 1,4,8,11-tetraazacyclotetradecane (cyclam) is presented. The complex showed a molar absorbtivity of 1.5?×?10⁴?L?mol^?1?cm^?1 at 379?nm. Under optimum experimental conditions, a pH of 4.5 and 1.960?×?10³?mg?L^?1 cyclam were selected, and all measurements were performed 10?min after mixing. Major cations and anions did not show any interference; Beer's law was applicable in the concentration range 0.2–20?mg?L^?1 with a detection limit of 0.001?mg?L^?1. The standard deviation in the determination is ±0.5?mg?L^?1 for a 15.0?mg?L^?1 solution (n?=?7). The described method provides a simple and reliable means for determination of Cr(VI) in real samples.     

Determination of Cysteine using the Fluorescence from a L-Tyrosine-Copper(II) Complex

A simple and sensitive method for the determination of cysteine is reported based on fluorescence quenching and recovery of L-tyrosine. At pH 10, copper(II) reacted with L-tyrosine to form a 1:1 complex that resulted in the quenching of L-tyrosine. However, the quenched fluorescence of L-tyrosine was recovered upon adding cysteine due to the strong affinity between these components. Under the optimized conditions, the recovered fluorescence was linearly proportional to the concentration of cysteine from 6.5?×?10^?7 to 4?×?10^?5?mol?L^?1 with a detection limit of 7.32?×?10^?8?mol?L^?1, demonstrating high sensitivity for the determination of cysteine. The mechanisms of fluorescence quenching and recovery were characterized and the method was used to determine cysteine in a pharmaceutical product with satisfactory results.     

Determination of 1-hydroxypyrene in human urine by a multi-wall carbon nanotubes-modified glassy carbon electrode

A multi-walled carbon nanotubes (MWNTs) modified glassy carbon electrode (MWNT-GCE) was used to study the electrochemical behaviour of1-hydroxypyrene (1-OHP) and applied to its determination. The results showed that the modified electrode had a strong adsorptive ability to 1-OHP and enhances its electrochemical signal. By square wave voltammetry, the linear relationship of 1-OHP was 6?×?10^?9???8?×?10^?7?mol?L^?1 with a linear correlation coefficient of 0.996, and the detection limit was 1?×?10^?10?mol?L^?1. Compared with other published methods, this newly proposed method possesses many advantages such as very low detection limit, fast response, low cost and simplicity. And this method was applied successfully in the determination of 1‐OHP in real human urine samples.     

Determination of three Tumor Biomarkers (Homovanillic Acid,Vanillylmandelic Acid,and 5‐Hydroxyindole‐3‐Acetic Acid) Using Flow Injection Analysis with Amperometric Detection

Flow injection analysis with amperometric detection (FIA‐AD) at screen‐printed carbon electrodes (SPCEs) in optimum medium of Britton‐Robinson buffer (0.04 mol ? L^?1, pH 2.0) was used for the determination of three tumor biomarkers (homovanillic acid (HVA), vanillylmandelic acid (VMA), and 5‐hydroxyindole‐3‐acetic acid (5‐HIAA)). Dependences of the peak current on the concentration of biomarkers were linear in the whole tested concentration range from 0.05 to 100 μmol ? L^?1, with limits of detection (LODs) of 0.065 μmol ? L^?1 for HVA, 0.053 μmol ? L^?1 for VMA, and 0.033 μmol ? L^?1 for 5‐HIAA (calculated from peak heights), and 0.024 μmol ? L^?1 for HVA, 0.020 μmol ? L^?1 for VMA, and 0.012 μmol ? L^?1 for 5‐HIAA (calculated from peak areas), respectively.     

Determination of phenylglyoxylic acid in urine using a multi-pumping flow system

In this work a simple, fast and fully automated analytical methodology for the spectrophotometric determination of phenylglyoxylic acid is proposed. Phenylglyoxylic acid is a metabolite of styrene that is excreted in urine, being used as an indicator of styrene occupational exposure. The developed procedure was based on the phenylglyoxylic acid ability to inhibit the formation of the peroxovanadium cation produced by the reaction between vanadate and H₂O₂. The analytical process was implemented in a multi-pumping flow system that employs multiple solenoid actuated micro-pumps as the only active components. This enabled the reproducible insertion and efficient mixing of low volumes of sample and reagents as well as the transportation of the sample zone towards detection. Thus an easily controlled, low cost, compact and reliable analytical system was implemented. A linear working range for phenylglyoxylic acid concentrations up to 700?mg?L^?1 (r ^2?=?0.995, n?=?7), was obtained, with a detection limit of 37?mg?L^?1. The system handles about 43 determinations per hour yielding precise results (relative standard deviation?<?5%, n?=?10). The developed methodology was applied to the determination of phenylglyoxylic acid in urine samples and the obtained results were in agreement with those furnished by the comparison method with relative percentage deviations lower than 6.6%.     

The electrochemistry of uric acid at a gold electrode modified with L-cysteine, and its application to sensing uric urine

The electrochemistry of uric acid at a gold electrode modified with a self-assembled film of L-cysteine was studied by cyclic voltammetry and differential pulse voltammetry. Compared to the bare gold electrode, uric acid showed better electrochemical response in that the anodic peak current is stronger and the peak potential is negatively shifted by about 100 mV. The effects of experimental conditions on the oxidation of uric acid were tested and a calibration plot was established. The differential pulse response to uric acid is linear in the concentration range from 1.0?×?10^?6 to ~?1.0?×?10^?4 mol?L^?1 (r?=?0.9995) and from 1.0?×?10^?4 to ~?5.0?×?10^?4 mol?L^?1 (r?=?0.9990), the detection limit being 1.0?×?10^?7 mol?L^?1 (at S/N?=?3). The high sensitivity and good selectivity of the electrode was demonstrated by its practical application to the determination of uric acid in urine samples.

Anodic Stripping Voltammetric Determination of Aurothiomalate in Urine Using a Screen‐Printed Carbon Electrode

This work describes an electroanalytical method for determining gold(I) thiomalate, aurothiomalate, widely used for treatment of reumatoid arthiritis, using a screen‐printed carbon electrode (SPCE). Aurothiomalate (AuTM) was determined indirectly at the same electrode by accumulating it first at ?1.5 V vs. printed carbon. At this potential in the adsorbed state, the AuTM is reduced to Au(0), which is then oxidized at two steps at ?0.22 V and +0.54 V on SPCE. Using optimized conditions of 60 s deposition time, ?1.5 V (vs. printed carbon) accumulation potential, 100 mV s^?1 scan rate, linear calibration graphs can be obtained by monitoring the peak at +0.54 V for AuTM in HCl 0.1 mol L^?1 from 1.43×10^?6 to 1.55×10^?4 mol L^?1. A limit of detection obtained was 6.50×10^?7 mol L^?1, and the relative standard deviation from five measurements of 3.0×10^?5 mol L^?1 AuTM is 4.5%. The method was successfully applied for AuTM determination in human urine sample.     

Simultaneous determination of trichloroethylene,perchloroethylene and trichloroacetic acid in human urine using solid-phase microextraction fibre coated with single-walled carbon nanotubes

A reliable and sensitive method for simultaneous determination of perchloroethylene (PCE), trichloroethylene (TCE), and trichloroacetic acid (TCA) in human urine by gas chromatography-mass spectrometry (GC/MS) is described after extraction and preconcentration by a new solid-phase microextraction (SPME) adsorbent. The potential of single-walled carbon nanotubes (SWCNTs) as SPME adsorbent for the pre-concentration of environmental pollutants has been investigated in recent years. This work was carried out to investigate the feasibility of SWCNTs as a headspace SPME adsorbent for the determination of chloroethylenes in human urine. SWCNTs were attached onto a stainless steel wire through an organic binder. Potential factors affecting the extraction efficiency, including extraction time, extraction temperature, desorption time, desorption temperature, and salinity were optimized. The developed method showed good performance. For PCE and TCE, calibration curves were linear (r ^{2 ?}≥?0.994) over the concentration ranges from 15 to 8000?ng?L^?1 and the limit of detection (LOD) at signal-to-noise (S/N) ratio of 3 was 5?ng?L^?1. The analytical procedure also involves derivatization of TCA with dimethyl sulfate, before headspace sampling. For TCA the linear range and LOD were 45-8000 (r ^{2 ?}≥?0.992) and 15?ng L^?1, respectively. In addition, a comparative study between the SWCNT and a commercial carboxen/polydimethylsiloxane (CAR/PDMS) SPME fibre for the determination of chloroethylenes in human urine was carried out. SWCNT fibre showed higher extraction capacity, better thermal stability (over 350°C) and longer life span (over 200 times) than the commercial CAR/PDMS fibre. The developed method was successfully applied to determine chloroethylenes in human urine samples. As the results indicated, the mean concentrations of TCE, PCE and TCA in exposed workers (dry-cleaning industry workers) were significantly greater than that of control group.     

Flow Injection Spectrophotometric Determination of Dipyrone in Pharmaceutical Formulations Using Fe(III) as Reagent

A flow injection spectrophotometric procedure with symmetric merging zones for dipyrone determination in pharmaceutical formulations is proposed. The determination is based on the formation of a blue complex (monitored at a wavelength of 642 nm) yield in the complexation reaction of dipyrone with Fe(III) in acid medium. Under optimum conditions, a calibration curve was obtained from 3.5 to 281 mg L^?1 with a detection limit of 2.8 mg L^?1 and the samples throughput was 80 h^?1. The analytical results obtained for commercial formulation samples by applying the proposed method were in good agreement with labeled values and those obtained by a comparative procedure at a 95% confidence level.     

Determination of Selenium by Single-Drop Microextraction and Diffuse Reflectance Infrared Spectroscopy

A simple and convenient assay based on single-drop microextraction with infrared spectroscopy is reported for the determination of selenium. The extraction conditions were carefully optimized and selenium was preconcentrated through single-drop microextraction in 1,2-dichloroethane containing N-hydroxy-N-phenyl-N′-(o-tolyl) benzimidamide. The method is selective and almost all common ions including molybdenum(VI), chromium(VI), and tungsten(VI) did not interfere with the isolation protocol. The selenite band at 875?±?2?cm^?1, which is assigned to the asymmetric vibrational stretch (υ₃), was used for the quantification of selenium. Low limits of detection and quantification of 2.0 and 6.6?µg?L^?1 demonstrate the sensitivity of the method. Good precision was evaluated by the standard deviation (2.0?µg?L^?1) and relative standard deviation (0.5%) for 8?µg?L^?1 was achieved for 10 measurements. The method was used to analyze human blood, urine, and water for selenium.     

Sensitive Simultaneous Determination of o-Nitrophenol and p-Nitrophenol in Water by Surfactant-Mediated Differential Pulse Voltammetry

A simple, low-cost and sensitive electroanalytical method was developed for the simultaneous determination of p-nitrophenol and o-nitrophenol isomers in water samples at a glassy carbon electrode (CGE) in the presence of cationic surfactant. The electrochemical behavior of p-nitrophenol and o-nitrophenol was studied by cyclic voltammetry (CV) in 0.1?mol L^?1 acetate/acetic acid buffer (pH 3.70) in the presence and absence of cetylpyridinium bromide. The resolution of overlapped cathodic peaks potentials (E_pc) of isomers was successfully improved in the presence of 100.0?µmol L^?1 cetylpyridinium bromide, thus making this approach ideal for the simultaneous determination of isomers. Under the optimized conditions in 0.05?mol L^?1 HEPES buffer at pH 7.0 using differential pulse voltammetry (DPV) at a scan rate of 45?mV s^?1, pulse amplitude of 220?mV and modulation time of 10?ms, limits of detection 0.59?µmol L^?1 for p-nitrophenol and 1.14?µmol L^?1 for o-nitrophenol were obtained with linear ranges from 2.0 to 60.0?µmol L^?1 and 3.0 to 60.0?µmol L^?1, respectively. The intraday precision was assessed as relative standard deviation (%) for 20.0 and 40.0?µmol L^?1 concentrations were 4.30% and 2.41% for p-nitrophenol and 4.87% and 2.20% for o-nitrophenol, respectively. The developed method was applied for the determination of the isomers in lake water samples. The accuracy was attested by comparison with high-performance liquid chromatography with diode array detection (HPLC-DAD) as a reference analytical technique. Recovery values ranging from 90.3% to 111.8% also attested to the accuracy of method for analysis of real samples.     

New extraction procedures for isolation of famotidine from aqueous samples

Liquid-liquid and solid-phase extraction procedures are proposed for famotidine isolation from aqueous samples. The isolation and spectrophotometric determination of famotidine is based on its complexation reaction with thymol blue. The composition of a complex between drug and reagent (1?:?1) was established. Dichloromethane and methanol were used as extraction solvents for LLE and SPE processes. Quantification of famotidine was done spectrophotometrically at 544?nm for dichloromethane or at 434?nm for methanolic extracts. The Beer law is obeyed in the famotidine concentration range 3?·?10^?5?mol?L^?1–2.0?·?10^?4?mol?L^?1 for LLE procedure and 2.0?·?10^?6?mol?L^?1–8.0?·?10^?5?mol?L^?1 for SPE.     

A new voltammetric sensor for the determination of sulfite in water and wastewater using modified-multiwall carbon nanotubes paste electrode

The electrochemical response of a modified-carbon nanotubes paste electrode with p-aminophenol was investigated as an electrochemical sensor for sulfite determination. The electrochemical behaviour of sulfite was studied at the surface of the modified electrode in aqueous media using cyclic voltammetry and square wave voltammetry. It has been found that under the optimum condition (pH 7.0) in cyclic voltammetry, the oxidation of sulfite occurs at a potential about 680?mV less positive than that of an unmodified-carbon nanotubes paste electrode. Under the optimized conditions, the electrocatalytic peak current showed linear relationship with sulfite concentration in the range of 2.0?×?10^?7–2.8?×?10^?4?mol?L^?1 with a detection limit of 9.0?×?10^?8?mol?L^?1 sulfite. The relative standard deviations for ten successive assays of 1.0 and 50.0?µmol?L^?1 sulfite were 2.5% and 2.1%, respectively. Finally, the modified electrode was examined as a selective, simple and precise new electrochemical sensor for the determination of sulfite in water and wastewater samples.     

Development of non-enzymatic strip for simple and selective determination of urea in water and biological samples

A simple and selective method for the determination of urea based on the paptode technique is described. The sensor was constructed by immobilizing an ionophore on a TLC strip. The procedure is based on the nucleophilic displacement of urea with tetrachloro-p-benzoquinone (chloranil) as an ionophore, and the formed violet-color product was detected using a flatbed scanner. The color of each spot was analyzed to red (R), green (G) and blue (B) values from 0 to 255 using a program written in visual basic (VB) programming language. The calibration graph obtained with the proposed sensor was linear over the range of 0.05?C10.00?mg?L^?1 with a detection limit of 0.01?mg?L^?1 for urea. Parameters such as pH and concentration of chloranil were optimized. The proposed sensor was successfully applied for the determination of urea in bovine serum, urine and tap water samples.