A rapid HPLC method for the determination of carboxylic acids in human urine using a monolithic column

A rapid HPLC method for the determination of carboxylic acids in urine samples using a Chromolith Performance RP/18e 100/4.6 with Chromolith Guard Cartridge RP/18e 10/4.6 (Merck KgaA, Darmstadt, Germany) was developed. The method facilitates the simultaneous determination of aromatic hydrocarbon metabolites mandelic acid (MA) and phenylglyoxylic acid (PGA) from styrene and ethylbenzene, hippuric acid (HA) from toluene and 2-, 3-, 4-methylhippuric acids (MHA) from xylene. 3-Hydroxybenzoic acid (3-HBA) was used as internal standard. A chromatographic run is completed within less than 5 min for styrene, ethylbenzene and toluene metabolites, and within 10 min for xylene metabolites. The detection limits are 9 mg L^–1 urine for MA, 1.25 mg L^–1 urine for PGA, 4.9 mg L^–1 urine for HA, 22 mg L^–1 urine for 2-MHA, and 18.5 mg L^–1 urine for 3-MHA.No significant differences of the MA, PGA and HA concentrations in human urine samples obtained by HPLC chromatography on LiChrosorb RP 18 and on Chromolith RP/18e columns were found. The results were evaluated by using ANOVA.Abbreviations MA mandelic acid - PGA phenylglyoxylic acid - HA hippuric acid - MHA methylhippuric acid - 3-HBA 3-hydroxybenzoic acid - ANOVA analyses of variance - GC gas chromatography - HPLC high-performance liquid chromatography     

Determination of B in body fluids by isotope dilution inductively coupled mass spectrometry with direct injection nebulization

The determination of B in small volumes of undigested blood plasma and urine by isotope dilution and high efficiency direct injection nebulization (DIN) inductively coupled plasma mass spectrometry (ICP-MS) is proposed. The C interference over ¹¹B was removed by precipitating the samples proteins. Samples aliquots of 1 ml were spiked with an enriched ¹⁰B solution and shaken during 1 h to attain the isotopic equilibrium. Thereafter, the sample proteins were denaturated with nitric acid and the supernatant was analyzed. This procedure was effective to reduce C concentrations in approximately 94%. Sample volumes of 50 μl were introduced into the ICP by the direct injection nebulizer producing transient signals lasting 30 s for B isotopes measurements. Precision of ¹⁰B/¹¹B measurements was characterized by relative standard deviation (RSD) lower than 1%. The instrumental mass discrimination factor was lower than 5%. Total B concentrations from 100 to 135 μg L⁻¹ in plasma and 0.499 to 3.021 mg L⁻¹ in urine samples were found. Reproducibility of triplicate samples was characterized by RSD<2.0% for plasma and lower than 1.3% for urine samples. Limit of detection (3σ) of 0.6 ng ml⁻¹ was calculated from synthetic blood plasma blank. Results of the denatured supernatant and digested plasma and urine samples were comparable at the 95% confidence level.     

Determination of macrolide antibiotics in porcine and bovine urine by high-performance liquid chromatography coupled to coulometric detection

A high-performance liquid chromatography method coupled to coulometric detection has been applied for the determination, in a single run, of up to eight macrolide antibiotics (erythromycin [ERY], tylosin [TYL], tilmicosin [TILM], spiramycin 2 [SPI 2], spiramycin 3 [SPI 3], josamycin [JOS], kitasamycin [KIT], and rosamicin [ROS]) in spiked porcine and bovine urine. Quantification was performed using matrix-matched calibration with roxithromycin (ROX) as the internal standard. The detection limits for each drug were below 3.5 ng injected (equivalent to an initial concentration below 0.07 mg L^–1) for porcine urine and below 5 ng injected (equivalent to an initial concentration below 0.10 mg L^–1) for bovine urine. Recoveries from urine samples spiked at three different concentrations within the linear range were not significantly dependent on concentration. The entire procedure provides average macrolide recoveries ranging from 69.7 to 96.6% for bovine urine and from 75.5 and 96.1% for porcine urine.     

Optimisation and validation of an automated solid phase extraction technique coupled on-line to enzyme-based biosensor detection for the determination of phenolic compounds in surface water samples

Summary A fully integrated screening system for phenolic compounds was developed incorporating on-line solid phase extraction, fractionation and biosensor detection. Two different types of biosensors, solid graphite and carbon paste electrodes incorporating the enzyme tyrosinase, were compared and used in the screening system. Interfacing of the solid phase extraction and fractionation with the biosensor detection was given special attention since the biosensors were not compatible with the organic modifier used for desorption of phenols from the solid phase extraction step. The system was validated with conventional analytical techniques. Surface water samples from the Ebro river were spiked with 1,10, and 25g L^–1 of catechol, phenol,p-cresol, respectively. Three out of seven samples were spiked and the correct samples were identified, containing phenols equivalent to the spiked concentrations.     

Determination of Trace Amount of Silver by Atomic-Absorption-Spectrometry-Coupled Flow Injection On-Line Coprecipitation Preconcentration Using DDTC–Copper as Coprecipitate Carrier

A flow injection on-line coprecipitation preconcentration system with diethyldithiocarbamate (DDTC) chelate of copper used as the coprecipitate carrier was coupled with flame atomic absorption spectrometry (FAAS) for the determination of trace silver. Silver was on-line coprecipitated with DDTC-Cu(II) in 0.5 moL · L⁻¹HCl, and the precipitate was collected in a knotted reactor. The precipitate was then dissolved by isobutyl methyl ketone and transported directly into the nebulizer–burner system of a flame atomic absorption spectrometer. A detection limit (3ς) of 0.6 μg · L⁻¹was achieved for a loading period of 30 s, a relative standard derivation of 2.0% was obtained for 11 determinations of 20 μg · L⁻¹Ag(I). Interference-free levels were 10 mg · L⁻¹for Cd²⁺, 50 mg · L⁻¹for Cu²⁺, 50 mg · L⁻¹for Mn²⁺, 25 mg · L⁻¹for Ni²⁺, 100 mg · L⁻¹for Pb²⁺, 50 mg · L⁻¹for Zn²⁺, 500 mg · L⁻¹for Fe³⁺, and 2000 mg · L⁻¹for Fe²⁺reduced from Fe³⁺by ascorbic acid. The developed method has been successfully applied to the determination of trace amount of silver in geological samples.     

Simultaneous determination of hydroquinone and catechol at PASA/MWNTs composite film modified glassy carbon electrode

A poly-amidosulfonic acid and multi-wall carbon nanotubes composite (PASA/MWNTs) modified electrode has been constructed by electropolymerization on glassy carbon electrode (GCE). The electrochemical behaviors of hydroquinone (HQ) and catechol (CC) were investigated using cyclic and differential pulse voltammetries (DPVs) at the prepared electrode. Separation of the reductive peak potentials for HQ and CC was about 120 mV in pH 6.0 phosphate buffer solution (PBS), which makes it suitable for simultaneous determination of these compounds. In the presence of 1.0 × 10⁻⁴ mol L⁻¹ isomer, the reductive peak currents of DPV are proportional to the concentration of HQ in the range of 6.0 × 10⁻⁶ to 4.0 × 10⁻⁴ mol L⁻¹, and to that of CC in the range of 6.0 × 10⁻⁶ to 7.0 × 10⁻⁴ mol L⁻¹. When simultaneously changing the concentration of both HQ and CC, the linear concentration range of HQ (or CC) is 6.0 × 10⁻⁶ to 1.0 × 10⁻⁴ mol L⁻¹ (or 6.0 × 10⁻⁶ to 1.8 × 10⁻⁴ mol L⁻¹), and the corresponding detection limits are 1.0 × 10⁻⁶ mol L⁻¹. The proposed method has been applied to simultaneous determination of HQ and catechol in water sample, and the results are satisfactory.     

Utilization of 2,6-bis(2-benzimidazolyl)pyridine to detect toxic benzene metabolites

The tridentate ligand 2,6-bis(2-benzimidazolyl)pyridine has the ability to detect toxic benzene metabolites such as phenol, hydroquinone, resorcinol, catechol and p-benzoquinone by simple techniques like UV/vis and fluorescence spectroscopy. The formation of a stable supramolecular complex between 2,6-bis(2-benzimidazolyl)pyridine and hydroquinone was confirmed by X-ray analysis.     

Human urine certified reference material CZ 6010: creatinine and toluene metabolites (hippuric acid and o-cresol) and a benzene metabolite (phenol)

A reference material for the biological monitoring of occupational exposure to toluene, benzene and phenol was prepared. O-cresol and hippuric acid (metabolites of toluene) are used for the biological monitoring of occupational exposure to toluene. Phenol, a metabolite of benzene, is used for the biological monitoring of exposure to benzene, but phenol can of course also be used as an indicator of exposure to phenol as well. The reference material (RM) used for the determination of these metabolites was prepared by freeze-drying pooled urine samples obtained from healthy persons occupationally exposed to toluene and those taking part in an inhalation experiment. Tests for homogeneity and stability were performed by determining urine concentrations of o-cresol, hippuric acid, creatinine and phenol. To investigate the stability of the RM, the urinary concentrations of o-cresol and phenol were monitored for eighteen months using GC and HPLC, while those of hippuric acid and creatinine were followed for five and six years, respectively, using HPLC. Analysis of variance showed that the concentrations did not change. The certified concentration values (and their uncertainties) of the substances in this reference material (phenol concentration c=6.46±0.58 mg l⁻¹; o-cresol concentration c=1.17±0.15 mg l⁻¹; hippuric acid concentration c=1328±30 mg l⁻¹; creatinine concentration c=0.82±0.10 g l⁻¹) were evaluated via the interactive statistical programme IPECA.     

Determination of moxifloxacin in tablets and human urine by square-wave adsorptive voltammetry

This work presents an electroanalytical methodology developed for square-wave voltammetry based in the electrochemical reduction in hanging mercury drop electrode (HMDE), which is simple, fast, reliable and sensitive for determination of moxifloxacin (MOXI) in tablets and spiked urine human samples. The support electrolyte that provided a more defined and intense peak current for MOXI determination was the phosphate buffer 0.04 mol l^{− 1} pH 8.0. In the best-optimized conditions the drug presented an only peak of reduction at − 1.38 V vs. Ag/AgCl, using an E_acc. of − 0.30 V. An LOD of 0.44 and 3.20 ng ml^{− 1} and an LOQ of 1.46 and 10.60 ng ml^{− 1} were found for the pure standard of moxifloxacin and in the presence of matrix, respectively. A good recovery was obtained for assay spiked urine samples and a good quantification of MOXI was achieved in a commercial formulation. The methodology proposed was more sensitive than the spectrofluorimetric and spectrophotometric method with precision and accuracy equivalent.     

Detection of ethanol in human body fluids by headspace solid-phase micro extraction (SPME)/capillary gas chromatography

Summary Ethanol has been found extractable from human whole blood and urine samples by headspace solid-phase micro extraction (SPME) with a Carbowax/divinylbenzene-coated fiber. After heating a vial containing the body fluid sample with ethanol, and isobutanol as internal standard (IS) at 70°C in the presence of (NH₄)₂SO₄, a Carbowax/divinylbenzene-coated SPME fiber was exposed in the headspace of the vial to allow adsorption of the compounds. The fiber needle was then injected into a middle-bore capillary gas chromatography (GC) port. The headspace SPME-GC gave intense peaks for both compounds; a small amount of background noises appeared, but did not interfere with the detection of the compounds. Recoveries of ethanol and IS were 0.049 and 0.026% for whole blood, respectively, and 0.054 and 0.085% for urine, respectively. The calibration curves for ethanol showed excellent linearity in the range of 80–5000 mg L^–1 for whole blood and 40–5000 mg L^–1 for urine; the detection limits for both samples were 20 and 10 mg L^–1, respectively. The data on actual determination of ethanol after the drinking of beer are also presented for two subjects.     

Application of Voltammetric Method of Total Chromium Determination in the Presence of Cupferron for Selective Determination of Cr(VI) in Water Samples

A voltammetric method of Cr(VI) determination in a flow system based on the combination of selective accumulation of the product of Cr(VI) reduction on hanging mercury drop electrode and a very sensitive method of chromium determination in the presence of cupferron previously described is proposed. The calibration graphs were linear from 3 × 10⁻⁹ to 3 × 10⁻⁸ and from 5 × 10⁻¹⁰ to 5 × 10⁻⁹ mol L⁻¹ for accumulation times of 120 and 600 s, respectively. The detection limit for the accumulation time of 600 s was 9 × 10⁻¹¹ mol L⁻¹. The relative standard deviation was 5.1% (n = 5) for Cr(VI) concentration 1 × 10⁻⁸ mol L⁻¹ and the accumulation time of 120 s. The influence of foreign ions commonly present in water samples is presented. The validation of the method was made by studying the recovery of Cr(VI) from spiked natural water samples.     

On-line molecularly imprinted solid phase extraction for the selective spectrophotometric determination of catechol

A molecularly imprinted polymer has been synthesized for a selective on-line catechol extraction, followed by its spectrophotometric determination in guarana powder, mate tea and tap water samples. A clean-up column, containing a methacrylic polymer + C₁₈ solid phase, was also used in order to enhance selectivity. The imprinted polymer was prepared by bulk polymerization using catechol as template and 4-vinylpyridine as the functional monomer. Permanganate solution was used as spectrophotometric reagent, where Mn(VII) was reduced to Mn(II) by catechol in an acid medium, causing color loss, which was monitored at 528 nm. Physical (extraction flow rate, elution flow rate, coil length) and chemical (nature and concentration of the eluent, potassium permanganate concentration) variables were optimized, and the selectivity was appraised using three molecules (4-chloro-2-methylphenol, 2-cresol, 2-methoxyphenol) similar to catechol. These molecules did not present interference in 1:8, 1:10 and 1:10 (catechol/concomitant) proportions, respectively. The analytical calibration curve ranged from 3.0 up to 100 μmol L^− 1 (r > 0.999; seven concentrations levels, n = 3) and the limits of detection (LOD) and quantification (LOQ) were 0.8 and 2.7 μmol L^− 1, respectively. Precision, expressed as RSD, was of 3.0% (20 μmol L^− 1, n = 10), and the analytical frequency was 15 h^− 1. Accuracy was checked by the HPLC technique and the results did not present significant difference at 95% confidence levels according to the t test.     

Development and critical comparison of greener flow procedures for nitrite determination in natural waters

Two greener procedures for flow-injection spectrophotometric determination of nitrite in natural waters were developed and critically compared. Replacement of toxic reagents, waste minimization and treatment were exploited to attend the standards of clean chemistry. The flow system was designed with solenoid micro-pumps in order to minimize reagent consumption and waste generation. The first procedure is based on the Griess diazo-coupling reaction with sulfanilamide and N-(1-naphthyl)ethylenediamine (NED) yielding an azo dye, followed by photodegradation of the low amount of waste generated based on the photo-Fenton reaction. The second procedure is based on the formation of iodine from nitrite and iodide in acid medium in order to avoid the use of toxic reagents. For Griess method, linear response was achieved up to 1.0 mg L^− 1, described by the equation A = − 0.007 + 0.460C (mg L^− 1), r = 0.999. The detection limit was estimated as 8 μg L^− 1 at the 99.7% confidence level and the coefficient of variation was 0.8% (n = 20). The sampling rate was estimated as 108 determinations per hour. The consumption of the most toxic reagent (NED) is reduced 55-fold and 20-fold in comparison to batch method and flow injection with continuous reagent addition, respectively. A colorless residue was obtained by in-line photodegradation with reduction of 87% of the total organic carbon content. The results obtained for natural water samples were in agreement with those achieved by the reference method at the 95% confidence level. For the nitrite–iodide method, linear response was observed up to 2.0 mg L^− 1, described by the equation A = − 0.024 + 0.148C (mg L^− 1), r = 0.999. The detection limit was estimated as 25 μg L^− 1 at the 99.7% confidence level and the coefficient of variation was 0.6% (n = 20). The sampling rate was estimated as 44 determinations per hour. Despite avoiding the use of toxic reagents, the nitrite–iodide method presented worst performance in terms of selectivity and sensitivity.     

Surface characterization and catalytic evaluation of copper-promoted Al-MCM-41 toward hydroxylation of phenol

The Mobil Composition of Matter No. 41 (MCM-41) containing Cu and Al with Si/Al ratios varying from 100 to 10 and 1 to 6 wt.% of Cu was synthesized under hydrothermal and impregnation conditions, respectively. The samples were characterized by nitrogen adsorption–desorption measurements, X-ray powder diffraction (XRD), Fourier transform infrared spectroscopy (FTIR), UV–Vis diffuse reflectance spectroscopy (UV–Vis DRS), temperature-programmed reduction (TPR), temperature-programmed desorption (TPD), and ²⁹Si and ²⁷Al magic-angle spinning–nuclear magnetic resonance (MAS–NMR) spectra. X-ray diffraction patterns indicate that the modified materials retain the standard MCM-41 structure. TPR patterns show the two-step reduction of Cu species. TPD study shows that Cu-impregnated Al-MCM-41 samples are more acidic than Al-MCM-41. From the MAS–NMR it was confirmed that most of the Al atoms are present tetrahedrally within the framework and some are present octahedrally in extraframework position. Impregnation of Cu shifted Al to the extraframework position. The catalytic activity of the samples toward hydroxylation of phenol in aqueous medium was evaluated using H₂O₂ as the oxidant at 80 °C. The effects of reaction parameters such as temperature, catalyst amount, amount of H₂O₂, and solvent were also investigated. Sample containing 4 wt.% copper-loaded Al-MCM-41-100 showed high phenol conversion (78%) with 68% catechol and 32% hydroquinone selectivity.     

In-field determination of nanomolar nitrite in seawater using a sequential injection technique combined with solid phase enrichment and colorimetric detection

A novel sequential injection method for the determination of nitrite at nanomolar level in seawater samples has been developed. The pink azo compound was formed based on the Griess reaction and quantitatively adsorbed onto a Sep-Pak C18 cartridge. The enriched azo compound was rinsed with water and ethanol (28%, v/v) in turn, and then eluted with an eluent containing 26.6% (v/v) ethanol and 0.108 mol L⁻¹ H₂SO₄. Finally the azo compound was measured using a spectrophotometer at 543 nm. Under the optimized conditions, the linear calibration ranges were 0.71–42.9 nmol L⁻¹ for a 150-mL sample and 35.7–429 nmol L⁻¹ for a 15-mL sample. The relative standard deviation of 8 measurements was 1.44% for 14.3 nmol L⁻¹ nitrite. For the 150 mL sample, the detection limit was estimated to be 0.1 nmol L⁻¹. The throughput of the method was about 4 samples per hour. The proposed method has been successfully applied to the in-field determination of nanomolar concentrations of nitrite in seawater.     

Kinetic Determination of Mercury(II) at Trace Level from Its Catalytic Effect on a Ligand Substitution Process

A catalytic kinetic method (CKM) is presented for the determination of mercury(II) based on its catalytic effect on the rate of substitution of N-methylpyrazinium ion (Mpz⁺) onto hexacyanoferrate(II). The progress of the reaction was monitored spectrophotometrically at 655 nm by registering the increase in absorbance of the product [Fe(CN)₅(Mpz]²⁻ under the reaction conditions: 5 × 10⁻³ mol L⁻¹ [Fe(CN)₆]⁴⁻), 5 × 10⁻⁵ mol L⁻¹ [Mpz⁺], T = 25.0 ± 0.1°C, pH 5.00 ± 0.02 and ionic strength, I = 0.1 mol L⁻¹ (KNO₃). Quantitative rate data at specified experimental conditions showed a linear dependence of the absorbance after fixed time A _t on the concentration of mercury(II) catalyst in the range 20.06–702.1 ng mL⁻¹. The maximum relative standard deviations and percentage errors for the determination of mercury(II) in the range of 20.06–200.6 ng mL⁻¹ were calculated to be 1.7 and 2.7% respectively. The detection limit was found to be 7.2 ng mL⁻¹ of mercury(II). Accuracy (expressed in terms of recoveries) was in the range of 98–103%. Figures of merit and interference due to many cations and anions was investigated and discussed. The applicability of the method was demonstrated by determining the mercury(II) in different synthetic samples and confirming the results using atomic absorption spectrophotometry. The proposed method allowed determination of mercury(II) in the range 20.06–702.1 ng mL⁻¹ with very good selectivity and an output of 30 samples h⁻¹.__________From Zhurnal Analiticheskoi Khimii, Vol. 60, No. 6, 2005, pp. 654–661.Original English Text Copyright © 2005 by Surendra Prasad.This article was submitted by the author in English.     

Rapid analysis of pyrethroids in whole urine by high-performance liquid chromatography using a monolithic column and off-line preconcentration in a restricted access material cartridge

A rapid high-performance liquid chromatography (HPLC) method using a monolithic column with UV detection at 238 nm was developed for the determination of fenpropathrin, betacyfluthrin, deltamethrin, and permethrin (cis and trans isomers) in whole urine. The method is based on the use of a monolithic chromatographic column and a restricted access material (RAM) cartridge for sample preparation. The mobile phase was water/acetonitrile (42:58 v/v), the flow rate was 3 mL min^–1, and chromatographic separation was carried out in 10 min. The separation of cis and trans isomers of permethrin was also possible under the above-mentioned conditions. Detection limits in reconstituted whole urine samples were between 0.9 g L^–1 for betacyfluthrin and 4.4 g L^–1 for fenpropathrin and trans-permethrin. Recoveries for urine samples spiked with different amounts of pyrethroids (between 19 g L^–1 and 75 g L^–1) were in the 70±6 to 90±7% range.     

Combined use of Pd and HF as chemical modifiers for the determination of total chromium in produced waters from petroleum exploration by ET AAS

This work reports the evaluation of the combined use of Pd and HF as chemical modifiers for the direct determination of total chromium in waters derived from petroleum exploration employing electrothermal atomic absorption spectrometry (ET AAS). Such waters, usually called as produced waters, have complex composition presenting a number of organic and inorganic substances. When obtained from offshore operations they also present high salinity. In order establish conditions for chromium measurement pyrolysis and atomization curves were built up in different media and employing Pd and HF as chemical modifiers. Also, a detailed study about calibration strategy was performed. At best conditions, pyrolysis and atomization temperatures were 1200 °C and 2600 °C, respectively, and 10 μL of a 500 mg L^− 1 Pd solution was added together with 10 μL of a 50% (v/v) HF solution on 20 μL of sample. Obtained results indicate that, in this kind of sample, chromium can be determined by standard addition method or employing external calibration with standard solutions prepared in 0.8 mol L^− 1 NaCl medium. In order to evaluate the accuracy of the procedure, a recovery test was performed with seven spiked samples of produced waters. The detection limit, quantification limit and the relative standard deviation in 0.8 mol L^− 1 NaCl were also calculated and the values found were 0.45 μg L^− 1, 1.5 μg L^− 1 and 6.0% (at 2.5 μg L^− 1 level), respectively.     

Enhanced sensitivity for Cu(II) by a salicylidine-functionalized polysiloxane carbon paste electrode

A new approach for decreasing the detection limit for a copper(II) ion-selective electrode (ISE) is presented. The ISE is designed using salicylidine-functionalized polysiloxane in carbon paste. This work describes the attempts to develop the electrode and measurements of its characteristics. The new type of renewable three-dimensional chemically modified electrode could be used in a pH range of 2.3–5.4, and its detection limit is 2.7 × 10⁻⁸ mol L⁻¹ (1.2 μg L⁻¹). This sensor exhibits a good Nernstian slope of 29.4 ± 0.5 mV/decade in a wide linear concentration range of 2.3 × 10⁻⁷ to 1.0 × 10⁻³ mol L⁻¹ of Cu(II). It has a short response time (8 s) and noticeably high selectivity over other Cu(II) selective electrodes. Finally, it was satisfactorily used as an indicator electrode in complexometric titration with EDTA and determination of copper(II) in miscellaneous samples such as urine and various water samples.     

Determination of benzene metabolites in urine of mice by solid-phase extraction and high-performance liquid chromatography.

A method was developed for quantitative measurement of trans,trans-muconic acid, catechol, hydroquinone and phenol in urine. Hydrolysis of esterified and glucuronized phenolic compounds was effected by specific enzymes. The hydrolysed mixture was purified and separated by solid-phase extraction with an anion exchanger, followed by extraction with diethyl ether. By using a clean-up procedure the natural background from mouse urine could be reduced, so that the detection limit of the metabolites was in the range 3-60 mg/l. Optimization of the chromatographic conditions resulted in a short high-performance liquid chromatography analysis time. Phenol had the longest retention time of about 10 min. The clean-up procedure could also be used for phenylmercapturic acid, an additional benzene metabolite, but for sensitive high-performance liquid chromatographic detection of phenylmercapturic acid other conditions are necessary.