Optimisation of sample treatment for arsenic speciation in alga samples by focussed sonication and ultrafiltration

A procedure for arsenic species fractionation in alga samples (Sargassum fulvellum, Chlorella vulgaris, Hizikia fusiformis and Laminaria digitata) by extraction is described. Several parameters were tested in order to evaluate the extraction efficiency of the process: extraction medium, nature and concentration (tris(hydroxymethyl)aminomethane, phosphoric acid, deionised water and water/methanol mixtures), extraction time and physical treatment (magnetic stirring, ultrasonic bath and ultrasonic focussed probe). The extraction yield of arsenic under the different conditions was evaluated by determining the total arsenic content in the extracts by ICP-AES. Arsenic compounds were extracted in 5 mL of water by focussed sonication for 30 s and subsequent centrifugation at 14,000 × g for 10 min. The process was repeated three times. Extraction studies show that soluble arsenic compounds account for about 65% of total arsenic.

An ultrafiltration process was used as a clean-up method for chromatographic analysis, and also allowed us to determine the extracted arsenic fraction with a molecular weight lower than 10 kDa, which accounts for about 100% for all samples analysed.

Speciation studies were carried out by HPLC–ICP-AES. Arsenic species were separated on a Hamilton PRP-X100 column with 17 mM phosphate buffer at pH 5.5 and 1.0 mL min⁻¹ flow rate. The chromatographic method allowed us to separate the species As(III), As(V), MMA and DMA in less than 13 min, with detection limits of about 20 ng of arsenic per species, for a sample injection volume of 100 μL. The chromatographic analysis allowed us to identify As(V) in Hizikia (46 ± 2 μg g⁻¹), Sargassum (38 ± 2 μg g⁻¹) and Chlorella (9 ± 1 μg g⁻¹) samples. The species DMA was also found in Chlorella alga (13 ± 1 μg g⁻¹). However, in Laminaria alga only an unknown arsenic species was detected, which eluted in the dead volume.     

Speciation of chromium in mineral waters and salinas by solid-phase extraction and graphite furnace atomic absorption spectrometry

A simple GF-AAS method for speciation analysis of chromium in mineral waters and salinas was developed. Cr(VI) species were separated from Cr(III) by solid-phase extraction with APDC (ammonium pyrrolidinedithiocarbamate). The APDC complexes were formed in the sample solution under proper conditions, adsorbed on Diaion HP-2MG resin and the resin was separated from the sample. After elution with concentrated nitric acid Cr(VI) was determined by GF-AAS. Total chromium was determined by GF-AAS directly in the sample and Cr(III) concentration was calculated as the difference between those results.

The detection limit of the method defined as 3 s of background variation was 0.03 μg l⁻¹ for Cr(VI) and 0.3 μg l⁻¹ for total chromium. RSD for Cr(VI) determination at the concentration of 0.14 μg l⁻¹ was 9%, and for total chromium at the concentration of 5.6 μg l⁻¹ was 5%. The recovery of Cr(VI) was in the range of 94–100%, dependently on type of the sample.

The investigation of recovery of the spiked Cr(VI) showed that at concentration levels near 1 μg l⁻¹ and lower recovery may be reduced significantly even by pure reagents that seem to be free from any reductants.     

Analysis of acrylamide in coffee and dietary exposure to acrylamide from coffee

An analytical method for analysing acrylamide in coffee was validated. The analysis of prepared coffee includes a comprehensive clean-up using multimode solid-phase extraction (SPE) by automatic SPE equipment and detection by liquid chromatography tandem mass spectrometry using electrospray in the positive mode. The recoveries of acrylamide in ready-to-drink coffee spiked with 5 and 10 μg l⁻¹ were 96±14% and 100±8%, respectively. Within laboratory reproducibility for the same spiking levels were 14% and 9%, respectively. Coffee samples (n = 25) prepared twice by coffee machines and twice by a French Press Cafetière coffee maker contained 8±3 μg l⁻¹ and 9±3 μg l⁻¹ acrylamide. Five ready-to-drink instant coffee prepared twice contained 8±2 μg l⁻¹. Hence, the results do not show significant differences in the acrylamide contents in ready-to-drink coffee prepared by coffee machine, French Press or from instant coffee. Medium roasted coffee contained more acrylamide (10 μg l⁻¹) than dark roasted coffee (5 μg l⁻¹). Males aged 35–45 years, drinking on average 1.1 l coffee per day are exposed to the highest doses of acrylamide from coffee. The dietary intake of acrylamide from coffee comprises, on an average, 10 μg day⁻¹ for males and 9 μg day⁻¹ for females aged 35–45 years. Probabilistic modelling of the exposure of Danish consumers (all adults) to acrylamide from coffee shows a mean exposure of 6.5 μg day⁻¹ and a 95 percentile of 18 μg day⁻¹.     

The use of microemulsion for determination of sodium and potassium in biodiesel by flame atomic absorption spectrometry

A new method for F AAS determination of sodium and potassium in biodiesel using water-in-oil microemulsion as sample preparation is proposed. The method was investigated for biodiesel produced from different sources, as soybean, castor and sunflower oil and animal fat and was also applied for vegetable oils. The optimized condition for microemulsion formation was 57.6% (w/w) of n-pentanol, 20% (w/w) of biodiesel or vegetable oil, 14.4% (w/w) of Triton X-100 and 8% (w/w) of water (aqueous standard of KCl or NaCl in/or diluted HNO₃). The optimized instrumental parameters were: aspiration rate of 2 mL min⁻¹ and the flame composition of 0.131 of C₂H₂/air ratio. For comparison purpose, the determination of sodium and potassium were also carried out according to European norms (EN 14108 and EN 14109, respectively). These norms are applied for determination of sodium and potassium in fatty acid methylic ester samples and consist in the sample dilution using organic solvent and determination by F AAS. The stability of microemulsified aqueous standards and samples was investigated and it was found to be stable for at least 3 days while the organic standard diluted with xylene showed a decrease around of 15% in the analytical signal in 1 h. The limits of detection were 0.1 μg g⁻¹ and 0.06 μg g⁻¹ and the obtained characteristic concentrations were 25 μg L⁻¹ and 28 μg L⁻¹ for sodium and potassium, respectively. The proposed method presented two times better limits of detection and better precision (0.4–1.0%) when compared with the dilution technique (1.5–4.5%). The accuracy of the method was evaluated through recovery tests and comparison with the results obtained by dilution technique. The recoveries ranged from 95% to 115% for biodiesel and 90% to 115% for vegetable oil samples. Comparison between the results obtained for biodiesel by both methods showed no significant differences at the 95% confidence level according to a Student's t-test. This study shows that the proposed method based on microemulsion as sample preparation can be applied as an efficient alternative for sodium and potassium determination in biodiesel samples.     

Atomic absorption spectrophotometric determination of trace copper in waters, aluminium foil and tea samples after preconcentration with 1-nitroso-2-naphthol-3,6-disulfonic acid on Ambersorb 572

An atomic absorption spectrophotometric method for the determination of trace copper after adsorption of its 1-nitroso-2-naphthol-3,6-disulfonic acid chelate on Ambersorb 572 has been developed. This chelate is adsorbed on the adsorbent in the pH range 1–8. The copper chelate is eluted with 5 ml of 0.1 mol l⁻¹ potassium cyanide and determined by flame atomic absorption spectrometry (FAAS). The selectivity of the proposed procedure was also evaluated. Results show that iron(III), zinc(II), manganese(II) and cobalt(II) at the 50 μg l⁻¹ level and sodium(I), potassium(I), magnesium(II), calcium(II) and aluminium(III) at the 1000 μg l⁻¹ level did not interfere. A high enrichment factor, 200, was obtained. The detection limit (3σ) of copper was 0.34 μg l⁻¹. The precision of the method, evaluated by seven replicate analyses of solutions containing 5 μg of copper was satisfactory and the relative standard deviation was 1.7%. The adsorption of copper onto Ambersorb 572 can formally be described by a Langmuir equation with a maximum adsorption capacity of 14.3 mg g⁻¹ and a binding constant of 0.00444 l mg⁻¹. The accuracy of the method is confirmed by analysing tomatoes leaves (NIST 1573a) and lead base alloy (NBS 53e). The results demonstrated good agreement with the certified values. This procedure was applied to the determination of copper in waters (tap, river and thermal waters), aluminium foil and tea samples.     

Investigation of equilibration and uncertainty contributions for the determination of inorganic mercury and methylmercury by isotope dilution inductively coupled plasma mass spectrometry

The mass fractions of Hg and methylmercury, in two certified reference materials, NIST2710 and DORM-2, have been determined by total and species-specific isotope dilution analysis (IDA), respectively, and uncertainty budgets for each analysis calculated. The mass fraction of Hg in NIST2710 was determined by ID using multicollector sector field inductively coupled plasma mass spectrometry (MC-SF-ICP-MS) whilst the mass fraction of methylmercury in DORM-2 was determined using HPLC coupled with quadrupole ICP-MS.

The extent of equilibration between the spike and the particulate bound mercury compounds was studied temporally by monitoring the ²⁰⁰Hg:¹⁹⁹Hg isotope amount ratio and by determining the total amount of Hg in the liquid phase. For the NIST2710 complete equilibration was only achieved when concentrated HNO₃ in combination with a microwave digestion was employed, and good agreement between the found (31.7±4.0 μg g⁻¹, expanded uncertainty k=2) and certified (32.6±1.8 μg g⁻¹) values was obtained. For DORM-2 complete equilibration of methylmercury between the liquid and solid phases was achieved when using 50:50 H₂O:CH₃OH (v/v) and 0.01% 2-mercaptoethanol as the solvent. Even though only 50% of the analyte was extracted into the liquid phase, complete equilibration was achieved, hence, the found methylmercury mass fraction (4.25±0.47 μg g⁻¹, expanded uncertainty k=2) was in good agreement with the certified value (4.47±0.32 μg g⁻¹).     

Biosorption of heavy metals on Aspergillus fumigatus immobilized Diaion HP-2MG resin for their atomic absorption spectrometric determinations

A solid phase extraction procedure based on biosorption of copper(II), lead(II), zinc(II), iron(III), nickel(II) and cobalt(II) ions on Aspergillus fumigatus immobilized Diaion HP-2MG has been investigated. The analytical conditions including amounts of A. fumigatus, eluent type, flow rates of sample and eluent solutions were examined. Good recoveries were obtained to the spiked natural waters. The influences of the concomitant ions on the retentions of the analytes were also examined. The detection limits (3sigma, N = 11) were 0.30 μg l⁻¹ for copper, 0.32 μg l⁻¹ for iron, 0.41 μg l⁻¹ for zinc, 0.52 μg l⁻¹ for lead, 0.59 μg l⁻¹ for nickel and 0.72 μg l⁻¹ for cobalt. The relative standard deviations of the procedure were below 7%. The validation of the presented procedure is performed by the analysis of three standard reference materials (NRCC-SLRS 4 Riverine Water, SRM 1515 Apple leaves and GBW 07605 Tea). The procedure was successfully applied for the determination of analyte ions in natural waters microwave digested samples including street dust, tomato paste, black tea, etc.     

As, Cd, Cr, Ni and Pb pressurized liquid extraction with acetic acid from marine sediment and soil samples

Rapid leaching procedures by Pressurized Liquid Extraction (PLE) have been developed for As, Cd, Cr, Ni and Pb leaching from environmental matrices (marine sediment and soil samples). The Pressurized Liquid Extraction is completed after 16 min. The released elements by acetic acid Pressurized Liquid Extraction have been evaluated by inductively coupled plasma-optical emission spectrometry. The optimum multi-element leaching conditions when using 5.0 ml stainless steel extraction cells, were: acetic acid concentration 8.0 M, extraction temperature 100 °C, pressure 1500 psi, static time 5 min, flush solvent 60%, two extraction steps and 0.50 g of diatomaceous earth as dispersing agent (diatomaceous earth mass/sample mass ratio of 2). Results have showed that high acetic acid concentrations and high extraction temperatures increase the metal leaching efficiency. Limits of detection (between 0.12 and 0.5 μg g^− 1) and repeatability of the over-all procedure (around 6.0%) were assessed. Finally, accuracy was studied by analyzing PACS-2 (marine sediment), GBW-07409 (soil), IRANT-12-1-07 (cambisol soil) and IRANT-12-1-08 (luvisol soil) certified reference materials (CRMs). These certified reference materials offer certified concentrations ranges between 2.9 and 26.2 μg g^− 1 for As, from 0.068 to 2.85 μg g^− 1 for Cd, between 26.4 and 90.7 μg g^− 1 for Cr, from 9.3 to 40.0 μg g^− 1 for Ni and between 16.3 and 183.0 μg g^− 1 for Pb. Recoveries after analysis were between 95.7 and 105.1% for As, 96.2% for Cd, 95.2 and 100.6% for Cr, 95.7 and 103% for Ni and 94.2 and 105.5% for Pb.     

Supported liquid membranes for the determination of vanillin in food samples with amperometric detection

A supported liquid membrane system has been developed for the extraction of vanillin from food samples. A porous PTFE membrane is impregnated with an organic solvent, which forms a barrier between two aqueous phases. The analyte is extracted from a donor phase into the hydrophobic membrane and then back extracted into a second aqueous solution, the acceptor. The determination (100–1400 μg ml⁻¹ vanillin) was performed using a PVC-graphite composite electrode versus Ag/AgCl/3MKCl at +0.850 V placed in a wall-jet flow cell as amperometric detector. The solid sample is directly placed in the membrane unit without any treatment, and the analyte was extracted from the sample, passes through the membrane and conduced to the flow cell by the acceptor stream. The limit of detection (3σ) was 44 μg ml⁻¹. The method was applied to the determination of vanillin (9–606 μg g⁻¹) in food samples.     

Multi-elemental analysis of non-food packaging materials by inductively coupled plasma-time of flight-mass spectrometry

Commercial non-food packaging materials of four different matrices (paper, low density polyethylene (LDPE), polyethylene-polypropylene (PE-PP) and high density polyethylene (HDPE)) were examined for the content of Cr, Ni, Cu, Zn, As, Mo, Cd, Sb, Ba, Hg, Tl, Pb and U. The examined samples (0.17–0.35 g) were digested in HNO₃ and H₂O₂ (papers, LDPE and PE-PP) and in HNO₃, H₂SO₄ and H₂O₂ (HDPE) using microwave assisted high pressure system. The inductively coupled plasma-time of flight-mass spectrometry (ICP-TOFMS) has been employed as the detection technique. All measurements were carried out using internal standardization. Yttrium and rhodium (50 ng g⁻¹) were used as internal standards. The detection and quantification limits obtained were in the range of 0.005 ng g⁻¹ (⁵²Cr) to 0.51 ng g⁻¹ (⁶⁶Zn) and 0.015 μg g⁻¹ (⁵²Cr) to 2.02 μg g⁻¹ (⁶⁶Zn) of dry mass, respectively. The evaluated contents (mg kg⁻¹) of particular elements in the examined materials were as follows: 0.22–219; <1.05–9.03; 1.25–112; <2.02–449; <0.98–<1.30; <0.36–2.06; <0.29–113; <0.22–44.1; <0.06–57.4; <0.66–<0.88; <0.08–0.24; <0.13–1222 and <0.08–0.44 for Cr, Ni, Cu, Zn, As, Mo, Cd, Sb, Ba, Hg, Tl, Pb and U, respectively.     

A liquid chromatographic method, with fluorometric detection, for the determination of enrofloxacin and ciprofloxacin in plasma and endometrial tissue of mares

The aim of this work was to develop and validate a simple and sensitive analytical method for determining enrofloxacin (EFX) and ciprofloxacin (CFX) in equine plasma and endometrial tissue samples, as a precursor to conducting pharmacokinetic/pharmacodynamic studies on equine endometritis This was achieved in the form of a liquid chromatographic procedure, with fluorometric detection, which also gave good separation of other fluoroquinolones including marbofloxacin (MFX), danofloxacin (DFX) and ofloxacin (OFX). Analytes were separated on a C₁₈ reversed phase column using an acidified mobile phase. The exact composition of the mobile phase differed for plasma (16% acetonitrile:methanol [13:1,v/v] 84% water containing 0.4% triethylamine and 0.4% phosphoric acid [35%]) and endometrial tissue (14% acetonitrile, 86% water, without methanol) samples. EFX and CFX were both detected at excitation and emission wavelengths of 294 and 500 nm, respectively. Prior to chromatography, EFX and CFX were purified by solid phase extraction from plasma, and a combination of solvent/solid phase extraction from endometrial tissue.

Mean absolute recoveries for EFX and CFX from plasma were 94.1 and 78.0%, respectively, and from endometrial tissue, 78.0 and 57.8%, respectively, with a percentage residual standard deviation (%R.S.D.) <10% in each case. Mean relative recoveries for EFX and CFX from plasma were 91.3 and 119.4%, respectively, and from endometrial tissue, 80.2 and 108.0%, respectively, with a %R.S.D. <20% in each case.

Standard curves constructed using blank plasma and endometrial tissue samples, spiked with authentic EFX and CFX in the ranges 0.005–10.0 μg mL⁻¹ and 0.05–10.0 μg g⁻¹, respectively, all showed acceptable linearity with correlation coefficients, r² ≥ 0.977. Mean intra- and inter-day precision (expressed as %R.S.D.) was <6 and <13%, respectively, with an associated accuracy (expressed as percentage relative error, %R.E.) of <20% for both analytes in both matrices. Acceptable precision and accuracy was also demonstrated at the pre-assigned LOQs of 0.005 μg mL⁻¹ for both EFX and CFX in plasma, and 0.05 μg g⁻¹ for both drugs in endometrial tissue. EFX and CFX were stable in both plasma and endometrial tissue for at least 60 days at −20 °C.     

Flow injection hydride generation electrothermal atomic absorption spectrometric determination of toxicologically relevant arsenic in urine

Analytical procedure for the determination of toxicologically relevant arsenic (the sum of arsenite, arsenate, monomethylarsonate and dimethylarsinate) in urine by flow injection hydride generation and collection of generated inorganic and methylated hydrides on an integrated platform of a transverse-heated graphite atomizer for electrothermal atomic absorption spectrometric determination (ETAAS) is elaborated. Platforms are pre-treated with 2.7 μmol of zirconium and then with 0.10 μmol of iridium which serve both as an efficient hydride sequestration medium and permanent chemical modifier. Arsine, monomethylarsine and dimethylarsine are generated from diluted urine samples (10–25-fold) in the presence of 50 mmol L⁻¹ hydrochloric acid and 70 mmol L⁻¹ l-cysteine. Collection, pyrolysis and atomization temperatures are 450, 500, 2100 and 2150 °C, respectively. The characteristic mass, characteristic concentration and limit of detection (3σ) are 39 pg, 0.078 μg L⁻¹ and 0.038 μg L⁻¹ As, respectively. The limits of detection in urine are ca. 0.4 and 1 μg L⁻¹ with 10- and 25-fold dilutions. The sample throughput rate is 25 h⁻¹. Applications to several urine CRMs are given.     

Determination of arsenic, lead, selenium and tin in sediments by slurry sampling electrothermal vaporization inductively coupled plasma mass spectrometry using Ru as permanent modifier and NaCl as a carrier

A procedure for the determination of As, Pb, Se and Sn in sediment slurries by electrothermal vaporization inductively coupled plasma mass spectrometry is proposed. The slurry, 1 mg ml⁻¹, is prepared by mixing the sample ground to a particle size 50 μm with 5% v/v nitric and 1% v/v hydrofluoric acids in an ultrasonic bath. The slurry was homogenized with a constant flow of argon in the autosampler cup, just before transferring an aliquot to the graphite furnace. The tube was treated with Ru as a permanent modifier, and an optimized mass of 1 μg of NaCl was added as a physical carrier. The pyrolysis temperature was optimized through pyrolysis curves, and a compromised temperature of 800 °C was used; the vaporization temperature was 2300 °C. The effect of different acid concentrations in the slurry on the analyte signal intensities was also evaluated. The accuracy of the method was assured by the analysis of certified reference sediments MESS-2, PACS-2 and HISS-1 from the National Research Council Canada, SRM 2704 and SRM 1646a from the National Institute of Standards and Technology and RS-4 from a round robin test, using external calibration with aqueous standards prepared in the same medium as the slurries. The obtained concentrations were in agreement with the certified values according to the Student's t-test for a confidence level of 95%. The detection limits in the samples were: 0.17 μg g⁻¹ for As; 0.3 μg g⁻¹ for Pb; 0.05 μg g⁻¹ for Se and 0.28 μg g⁻¹ for Sn. The precision found for the different sediment samples, expressed as R.S.D. was 1–8% for As, 2–9% for Pb, 6–12% for Se and 3–8% for Sn (n=5).     

Reverse flow injection spectrophotometric determination of iron(III) using chlortetracycline reagent

A simple reversed flow injection colourimetric procedure for determining iron(III) was proposed. It is based on the reaction between iron(III) with chlortetracycline, resulting in an intense yellow complex with a suitable absorption at 435 nm. A 200 μl chlortetracycline reagent solution was injected into the phosphate buffer stream (flow rate 2.0 ml min⁻¹) which was then merged with iron(III) standard or sample in dilute nitric acid stream (flow rate 1.5 ml min⁻¹). Optimum conditions for determining iron(III) were investigated by univariate method. Under the optimum conditions, a linear calibration graph was obtained over the range 0.5–20.0 μg ml⁻¹. The detection limit (3σ) and the quantification limit (10σ) were 0.10 and 0.82 μg ml⁻¹, respectively. The relatives standard deviation of the proposed method calculated from 12 replicate injections of 2.0 and 10.0 μg ml⁻¹ iron(III) were 0.43 and 0.59%, respectively. The sample throughput was 60 h⁻¹. The proposed method has been satisfactorily applied to the determination of iron(III) in natural waters.     

Kinetic spectrophotometric method for rapid determination of trace formaldehyde in foods

A simple and sensitive kinetic-spectrophotometric method was developed for the determination of ultra trace amount of formaldehyde in food samples. The method was based on the oxidation of rhodamine B (RhB) by potassium bromate in sulfuric acid medium (formaldehyde as catalyst). The reaction was monitored by measuring the decrease in absorbance of the dye at 515 nm after 6 min. The developed method allowed the determination of formaldehyde in the range of 10–100 μg L⁻¹ with good precision, accuracy and the detection limit was down to 2.90 μg L⁻¹. The relative standard deviations for the determination of 10 and 60 μg L⁻¹ of formaldehyde were 3.0% and 1.9% (n = 10), respectively. The method was found to be sensitive, selective and was applied to the determination of formaldehyde in foods with satisfactory results.     

Enhancement of the chemiluminescence of penicillamine and ephedrine after derivatization with aldehydes using tris(bipyridyl)ruthenium(II) peroxydisulfate system and its analytical application

A novel sequential injection (SI) method was developed for the determination of penicillamine (PA) and ephedrine (EP) based on the reaction of these drugs with tris(bipyridyl)ruthenium(II) (Ru(bpy)₃²⁺) and peroxydisulfate (S₂O₈²⁻) in the presence of light. Derivatization of PA and EP with aldehydes has resulted in a significant enhancement of the chemiluminescence emission signal by at least 25 times for PA and 12 times for EP, leading to better sensitivities and lower detection limits for both drugs. The instrumental setup utilized a syringe pump and a multiposition valve to aspirate the reagents, (Ru(bpy)₃²⁺ and S₂O₈²⁻), and a peristaltic pump to propel the sample. The experimental conditions affecting the derivatization reaction and the chemiluminescence reaction were systematically optimized using the univariate approach. Under the optimum conditions linear calibration curves between 0.2–24 μg mL⁻¹ for PA and 0.2–20 μg mL⁻¹ for EP were obtained. The detection limits were 0.1 μg mL⁻¹ for PA and 0.03 μg mL⁻¹ for EP. The procedure was applied to the analysis of PA and EP in pharmaceutical products and was found to be free from interferences from concomitants usually present in these preparations.     

Titanium as a chemical modifier for the determination of cobalt in marine sediments

The determination of cobalt in marine sediments by electrothermal atomic absorption spectrometry was studied using no modifier and magnesium and titanium as modifiers. Titanium is one of the major sediment constituents, which widely affects the cobalt determination and it was studied as a chemical modifier since it was the only concomitant that increased the cobalt signal in the concentration range usually found in sediments. The performance of Mg and Ti as chemical modifiers was compared relative to maximum pyrolysis and atomization temperatures, linear calibration range, sensitivity and matrix effects. The pyrolysis curves showed that the analyte could be stabilized up to 1400 °C when either Ti or Mg(NO₃)₂ was present, while only 1000 °C could be used in the absence of a modifier. The optimum atomization temperature was 2500 °C in all cases. Analytical curves were compared using no modifier, 5 μg Ti and 100 μg Mg(NO₃)₂ as modifiers, and the linear range found was up to approximately 4 ng Co whether a modifier was used or not. With Ti as a chemical modifier, analytical curves for cobalt in aqueous solution and in a synthetic matrix resulted in the same sensitivity (m₀=55 pg), whereas the use of Mg led to characteristic mass values of 59 and 72 pg in aqueous solution and in a synthetic matrix, respectively, showing some matrix effect. The detection limits (3σ, n=10) were 0.4 μg g⁻¹ using no modifier and 0.3 μg g⁻¹ with Ti as a modifier in the original matrix. A reference estuarine sediment NIST 1646 with a non-certified content of 10.5 μg g⁻¹ Co was analyzed and the found value of 10.9±2.4 μg g⁻¹, (n=3), using Ti as chemical modifier and calibration against aqueous standards, was in good agreement with the recommended value.     

Analytical procedures for the determination of selected major (Al, Ca, Fe, K, Mg, Na, and Ti) and trace (Li, Mn, Sr, and Zn) elements in peat and plant samples using inductively coupled plasma-optical emission spectrometry

A simple, robust and reliable analytical procedure for the determination of Al, Ca, Fe, K, Li, Mg, Mn, Na, Sr, Ti, and Zn in peat and plant materials by inductively coupled plasma-optical emission spectrometry (ICP-OES) was developed. A microwave heated high pressure autoclave was used to digest powdered sample aliquots (approximately 200 mg) with different acid mixtures including nitric acid (HNO₃), tetrafluoroboric acid (HBF₄) and hydrogen peroxide (H₂O₂). The optimized acid mixture for digestion of plant and peat samples consisted of 3 mL HNO₃ and 0.1 mL HBF₄, in addition to H₂O₂ which was sub-boiled into the PTFE digestion tubes during heating of the autoclave. Using HNO₃ alone, recoveries of Al and Ti were too low by 40 and 160%, respectively, because HNO₃ could not fully liberate the analytes of interest from the silicate fraction of the plant and peat matrix. However, for all other elements (such as Mn, Sr, and Zn), the use of HBF₄ was less critical. The accuracy of the analytical procedure developed was evaluated with peat and plant reference materials of different origin and composition. The ICP-OES instrument was optimized using solutions of plant reference materials considering RF power, nebulizer pressure, auxiliary gas flow and rinse time. Scandium was used as an online internal standard (IS) as it provided accurate results and showed less than 3% drift in sensitivity over time which was lower compared to other potential IS such as Rh (20%) and In (6%). The combination of most sensitive and less sensitive wavelengths allowed to obtain low detection limits and highest possible dynamic range. The achieved procedure detection limits ranged from 0.05 μg g⁻¹ (Li) to 15 μg g⁻¹ (Ca) and allowed a precise quantification of all elements. Comparative X-ray fluorescence spectrometric measurements of solid peat and plant samples generally agreed well with results obtained by digestion/ICP-OES. To overcome interferences caused by Na, K, and Li, a solution of 10 μg g⁻¹ CsCl₂ was successfully used as an ionization buffer. The good agreement between the found and certified concentrations in plant and peat reference materials indicates that the developed analytical procedure is well suited for further studies on the fate of major elements in plant and peat matrices.     

Monoclonal antibody-based ELISA for the quantification of nitrofuran metabolite 3-amino-2-oxazolidinone in tissues using a simplified sample preparation

A sensitive and specific monoclonal ELISA for the determination of tissue bound furazolidone metabolite 3-amino-2-oxazolidinone (AOZ) is described. The procedure enables the detection of AOZ in matrix supernatant after homogenisation, protease treatment, acid hydrolysis and derivatisation of AOZ released from the tissue by o-nitrobenzaldehyde. The formed p-nitrophenyl 3-amino-2-oxazolidinone (NPAOZ) is determined by ELISA calibrated with matrix-matched standards in the concentration range of 0.05–5.0 μg I⁻¹. The assay was validated according to criteria set down by Commission Decision 2002/657/EC for the performance and validation of analytical methods for chemical residues. Detection capability, set on the basis of acceptance of no false negative results, was 0.4 μg kg⁻¹ for shrimp, poultry, beef and pork muscle. This sensitivity approaches the established confirmatory LC–MS/MS able to quantify tissue-bound AOZ at levels as low as 0.3 μg kg⁻¹. An excellent correlation of results obtained by ELISA and LC/MS–MS within the concentration range 0–32.1 μg kg⁻¹ was found in the naturally contaminated shrimp samples (r = 0.999, n = 8). A similar correlation was found for the incurred poultry samples within the concentration range of 0–10.5 μg kg⁻¹ (r = 0.99, n = 8).     

Capillary liquid chromatography of chlorophenoxy acid herbicides and their esters in apple juice samples after preconcentration on a cation exchanger based on polydivinylbenzene-N-vinylpyrrolidone

A capillary liquid chromatography (cLC) method with gradient elution has been used to determine chlorophenoxy acid herbicides: 2,4-dichlorophenoxyacetic acid, 4-chloro-2-methylphenoxyacetic acid, 2-(2,4-dichlorophenoxy)propanoic acid, 2-(4-chloro-2-methylphenoxy)propanoic acid, 4-(2,4-dichlorophenoxy)butanoic acid, 4-(4-chloro-2-methylphenoxy)butanoic acid, 2-(2,4,5-trichlorophenoxy)propanoic acid, 2,4-dichlorophenoxyacetic-1-methyl ester and 2,4-dichlorophenoxyacetic-1-butyl ester in spiked apple juice samples with amounts between 0.025 and 0.150 mg kg(-1) of each herbicide. Clean-up and preconcentration of acid and esters were carried out in an Oasis MCX polymer. Detection limits obtained by cLC, between 0.005 and 0.018 mg kg(-1), allowed the determination of chlorophenoxy acids and their esters in apple juice samples around the levels permitted by the European Regulations, with recoveries in the range 84-99% and RSDs between 1 and 4%.