Chromotropic acid,a fluorogenic chelating agent for aluminium(III)

Complexation of aluminium(III) with the fluorogenic ligand chromotropic acid (4,5-dihydroxynaphthalene-2,7-disulfonic acid) has been revisited with the aim of using enhancement of the fluorescence intensity as an analytical tool. Complexation at the optimum pH4 was shown to lead to a 1:1 complex with a stability constant log ₁₁₀=18.4±0.7. The fluorogenic effect was thoroughly investigated. Nearly selective excitation of the chelate rather than the ligand could be achieved at wavelengths longer than 360 nm. For analytical purposes the main interfering ion was Ga³⁺. The strongest competing ligand was shown to be citric acid. Competitive complexation by acetate or formate ions can also make their use in a buffer at the usual concentration, 0.2 mol L^–1, questionable, whereas a 10^–2 mol L^–1 formic acid buffer was shown to be a good alternative. The calibration plot showed that the dependence of response on Al(III) concentration was linear up to 500 g L^–1; the detection limit was 0.65 g L^–1 (3SD _blank, n=10, SD=±1.4% at 10 g L^–1 and ±0.8% at 100 g L^–1). The analytical procedure was successfully applied to several samples of tap water and the results were in good agreement with those from AAS determination.     

Determination of Triphenyltin and Its Metabolite Diphenyltin in Culture Medium by High-Performance Liquid Chromatography with UV detection

A method for the determination of triphenyltin and diphenyltin was developed by reversed-phase high-performance liquid chromatography with UV detection. Triphenyltin and diphenyltin were separated using a reversed-phase Symmetry C₁₈ column (150 × 3.9 mm, 5 m) with tetrahydrofuran-water-acetonitrile-glacial acetic acid (13:25:5:7, v/v) containing 0.05% triethylamine and 1.0% sodium acetate as mobile phase at 0.50 mL min^–1 and detection at 257 nm. The calibration curves were linear from 0.26 mol L^–1 to 1100 mol L^–1 for triphenyltin with a correlation coefficient of 0.9999 (n=12) and from 0.60 mol L^–1 to 1200 mol L^–1 for diphenyltin with a correlation coefficient of 0.9991 (n=12), respectively. The detection limits of triphenyltin and diphenyltin were 0.2 mol L^–1 and 0.4 mol L^–1, respectively. The method was successfully applied to the determination of triphenyltin and its metabolite diphenyltin in culture medium. The recoveries of triphenyltin and diphenyltin were in the ranges of 97.7% to 103.3% and 85.5% to 91.6%, respectively.     

Platinum concentration in silicone breast implant material and capsular tissue by ICP-MS

Inductively coupled plasma-mass spectrometry (ICP-MS) was used to determine the concentration of platinum (Pt) in silicone breast implant gel (range, 0.26–48.90 g g^–1 Pt; n=15), elastomer (range, 3.05–28.78 g g^–1 Pt; n=7), double lumen (range, 5.79–125.27 g g^–1 Pt; n=7), foam (range, 5.79–8.36 g g^–1 Pt; n=2), and capsular tissue (range, 0.003–0.272 g g^–1 Pt; n=15). The results show that very high levels of Pt are present in the encasing elastomer, double lumen, and foam envelope materials. Silicone breast implants can be a source of significant Pt exposure for individuals with these implants.     

Development and application of a simple routine method for the determination of selenium in serum by octopole reaction system ICPMS

The aim of the study was to develop an inductively coupled plasma mass spectrometry (ICPMS) method for robust and simple routine determination of selenium in serum. Polyatomic interferences on ⁷⁶Se, ⁷⁷Se, and ⁷⁸Se were removed by applying an octopole reaction system ICPMS with the reaction cell pressurized with H₂ gas. We developed a novel simple optimization routine for the H₂ gas flow based on a signal-to-noise ratio (SNR) calculation of the selenium signal measured in a single selenium standard. The optimum H₂ flow was 2.9 mL min^–1. The selenium content in serum was determined after a 50-fold dilution with 0.16 M HNO₃ and quantified by using addition calibration and gallium as an internal standard. The method detection limit was 0.10 g L^–1 for ⁷⁶Se and ⁷⁸Se and 0.13 g L^–1 for ⁷⁷Se. Human serum samples from a case-control study investigating if selenium was associated with risk of colorectal adenoma were analyzed. The average selenium concentration for the control group (n=768) was 137.1 g L^–1 and the range was 73.4–305.5 g L^–1. The within-batch repeatability (a batch is ten samples) estimated from 182 replicate analyses was 6.3% coefficient of variation (CV), whereas the between-batch repeatability was 7.4% CV estimated from 361 replicates between batches. The method accuracy was evaluated by analysis of a human serum certified reference material (Seronorm Serum level II, Sero A/S, Norway). There was a fairly good agreement between the measured average of 145±3 g L^–1 (n=36) and the certified value of 136±9 g L^–1. In addition the method was successfully applied for analysis of zinc serum concentrations without further optimization. For the Seronorm certified reference material a value of 911±75 g L^–1 (n=31) for zinc was obtained, which corresponds well to the certified zinc value of 920±60 g L^–1.     

Isocratic high-performance liquid chromatographic determination of plasma adenosine

Summary Due to manifold physiological and cardioprotective actions of adenosine, the demand for a simple but accurate method to determine its concentration in plasma is increasing. The aim of this study was firstly to develop a simple isocratic method instead of the gradient elution or peak-shifting techniques used earlier and secondly to check conflicting data on the composition of stop-solution, added to the sample in order to prevent changes in adenosine concentration. Isocratic elution improved signal to noise ratio and concentrations of 100 mol L^–1 dipyridamole and 2.5 mol L^–1 erythro-9(2-hydroxy-3-nonyl)adenine in the blood sample effectively prevented both adenosine formation and degradation, even without the use of a 5-ecto-nucleotidase inhibitor. Lowering the concentration of dipyridamole to 25 mol L^–1 caused more than a tenfold increase of adenosine concentration in two out of five cases and even 100 mol L^–1 dipyridamole alone is not sufficient to inhibit adenosine deaminase in blood samples.     

Photometric detection of cyclodextrins in liquid chromatography by using iodine generated electrochemically in-situ

A method has been developed for photometric detection of cyclodextrins (CD) in liquid chromatography using iodine (I₂) generated electrochemically in-situ. Iodide ion in the mobile phase was electrochemically oxidized to I₂ which was subsequently reacted with I^–, in an electrochemical flow cell, forming I₃^–. The absorbance of I₃^– was found to be greatly enhanced when CD were present in the mobile phase. The absorbance enhancement was caused by the change in the mole fraction of I₃^–, because of the inclusion reaction of I₃^– with CD. On the basis of this phenomenon, CD were detected by means of a photodiode-array UV–visible detector positioned downstream of the electrochemical flow cell. The signals were found to be linearly dependent on CD concentration. Because the formation constants of I₃^– with CD decrease in the order -CD>-CD>-CD, -CD was most detectable by the method. Detection limits were 1.0 mol L^–1 for -CD, 65 mol L^–1 for monoG1--CD, 100 mol L^–1 for -CD, and 200 mol L^–1 for -CD.     

Chromatographic determination of D-amino acids as native constituents of vegetables and fruits

Summary Free D-amino acids (D-AA) were detected as native constituents in juices of vegetables (cultivars of cabbage, tomato, carrot, garlic) and fruits (organes, clementine, grapefruit, lemon, apples, pear, grapes) using gas chromatography (GC) or high-performance liquid chromatography (LC). For investigation by GC, AA enantiomers were converted into theirN(O)-pentafluoropropionyl 2-propyl esters and resolved on a Chirasil-L-Val capillary column. For determination by LC, precolumn derivatization of AA enantiomers usingo-phthaldialdehyde together with the chiral thiolsN-isobutyryl-L-cysteine orN-isobutyryl-D-cysteine and fluorescence detection of the diastereomeric isoindole derivatives, resolvable on an octadecylsilyl stationary phase, were used. D-Ala (0.6–3.8%) was detected in all freshly pressed plant juices usually in the highest relative amounts. Other D-AA detected were D-Asx (0.1–1.9%), D-Glx (0–1.3%), D-Ser (0–1.7%), D-Arg (0.4–1.2%, in grapes, orange, grapefruit, and clementine) and D-Leu and D-Val (1% in cabbage). Absolute amounts of native D-AA were totally 28–57 mol L^–1 in fruit juices, 14.5 mol L^–1 in a tomato juice and 8.5 mol L^–1 in a carrot juice.Presented in part as lecture at 3rd International Congress on Amino Acids, Peptides and Analogues, August 23–27, 1993, Vienna; and as posters at 31st Scientific Meeting of German Society of Nutrition, Giessen, March 17th and 18th, 1994 [19]; and at Analytica Conference, April 19–22, 1994, Munich [20].     

Determination of oxaliplatin in human plasma and plasma ultrafiltrate by graphite-furnace atomic-absorption spectrometry

A method for sensitive determination of the anti-cancer agent oxaliplatin in human plasma and human plasma ultrafiltrate (pUF) is presented. The method is based on the quantification of platinum by graphite-furnace atomic-absorption spectrometry, with Zeeman correction and an atomisation temperature of 2,700°C. Sample pretreatment involves dilution of the samples with a solution containing 0.15 mol L^–1 NaCl and 0.20 mol L^–1 HCl in water. Validation was performed in accordance with the most recent FDA guidelines for bioanalytical method validation. All results were within requirements. The validated ranges of quantification were 0.10–400 mol L^–1 for human pUF and 0.50–400 mol L^–1 for plasma. The assay is now successfully used to support pharmacokinetic studies of cancer patients treated with oxaliplatin.     

Determination of Endocrine Disruptors in Environmental Water Samples by Stir Bar Sorptive Extraction-Liquid Desorption - Large Volume Injection-Gas Chromatography

A method based on stir bar sorptive extraction with liquid desorption combined with gas chromatography and mass spectrometry detection has been developed to determine a group of endocrine disruptors in water samples. Large volume injection was used with a programmed temperature vaporiser injector in gas chromatography to enhance sensitivity. The parameters affecting stir bar sorptive extraction and large volume injection were optimised. The limits of quantification in the full scan mode were between 0.02 and 0.2 g L^–1 and the limits of detection were between 0.005 and 0.02 g L^–1 for river water samples. The reproducibility between days of the method (n=3) for river water samples spiked at 0.2 g L^–1 was below 15%. The performance of the method was checked with several water samples from the sea, and effluent and influent sewage treatment plants. We found 4-tert-octylphenol, benzylbutyl phthalate and bis(2-ethylhexyl) adipate in all the water samples analysed at levels between 0.02–14.04 g L^–1. Diazinon was found in only one effluent wastewater sample at 0.16 g L^–1.Acknowledgements This work was supported by the Ministerio de Ciencia y Tecnologia (projects AMB1999-0875 and PPQ2001-1805-CO3). We would like to thank Dr P. Sandra for kindly providing the stir bars.     

Determination of Benzimidazole Fungicides by HPLC with Fluorescence Detection After Micellar Extraction

An analytical method was developed to determine the benzimidazole fungicides and their residues (benomyl, carbendazim, thiabendazole and fuberidazole) in real water samples. Analyses were performed by reverse phase (RP) HPLC with direct fluorescence detection with mobile phase methanol:water, 40:60 (v/v) with 0.6% (v/v) ammonia. The extraction of analytes from water samples was performed with the use of micellar systems. Specifically, oligoethylene glycol monoalkyl ether (Genapol X-080) and polyoxyethylene 10 lauryl ether (POLE) were used as extractants. The recoveries of fungicides obtained in spiked water samples ranged from 68% to 94% for Genapol and from 68% to 96% for POLE. The limit of detection (LOD) was lower than 6 g L^–1 for carbendazim, 7 g L^–1 benomyl, 0.15 g L^–1 for thiabendazole and 0.01 g L^–1 for fuberidazole in both surfactants.     

Determination of phthalate monoesters in human milk,consumer milk,and infant formula by tandem mass spectrometry (LC–MS–MS)

Daily exposure of humans to phthalates may be a health risk because animal experiments have shown these compounds can affect the differentiation and function of the reproductive system. Because milk is the main source of nutrition for infants, knowledge of phthalate levels is important for exposure and risk assessment. Here we describe the development and validation of a quantitative analytical procedure for determination of phthalate metabolites in human milk. The phthalate monoesters investigated were: monomethyl phthalate (mMP), monoethyl phthalate (mEP), mono-n-butyl phthalate (mBP), monobenzyl phthalate (mBzP), mono-(2-ethylhexyl) phthalate (mEHP), and monoisononyl phthalate (mNP). The method is based on liquid extraction with a mixture of ethyl acetate and cyclohexane (95:5) followed by two-step solid-phase extraction (SPE). Detection and quantification of the phthalate monoesters were accomplished by high-pressure liquid chromatography using a Betasil phenyl column (100 mm×2.1 mm×3 m) and triple tandem mass spectrometry (LC–MS–MS). Detection limits were in the range 0.01 to 0.5 g L^–1 and method variation was from 5 to 15%. Analysis of 36 milk samples showed that all these phthalates were present, albeit at different concentrations. Median values (g L^–1) obtained were 0.11 (mMP), 0.95 (mEP), 3.5 (mBP), 0.8 (mBzP), 9.5 (mEHP), and 101 (mNP). We also analysed seven samples of consumer milk and ten samples of infant formula. Only mBP and mEHP were detected in these samples, in the ranges 0.6–3.9 g L^–1 (mBP) and 5.6–9.9 g L^–1 (mEHP).     

New books

Summary Micromolar analyses of the nitrogen species NH₃, NO ₂ ^– , and NO ₃ ^– in soil and other samples are usually accomplished by extracting several samples and testing each for a different species. This procedure is not viable when the quantity of the initial sample is limited. An improved method of separating and analysing for ammonia NH₃(aq), nitrite NO ₂ ^– (aq), and nitrate NO ₃ ^– (aq) from a single small sample with concentrations of 0–50 mol/l is reported. No interferences or carryovers among the three nitrogen containing species were found. Uncertainties were ±2–5 mol/l and accuracies with respect to standards were ±3 mol/l.     

Simultaneous Determination of Four Active Components in a Compound Formulation by Liquid Chromatography

Summary A rapid and accurate LC method is described for simultaneous determination of pseudoephedrine hydrochloride (PSE), acetaminophen (AMP), dextromethorphen hydrobromide (DEX), and diphenhydramine hydrochloride (DPH) in a compound formulation. Chromatographic separation of the four drugs was achieved on a Hypersil CN column (150 mm × 4.6 mm, 5 m particle) by use of a mobile phase comprising a mixture of 3 mM ion-pairing solution, 2% aqueous triethylamine solution, and 2 M phosphoric acid, 68:48:88 (v/v), pH 3.0, delivered at 1.0 mL min^–1. Compounds were detected at 215 nm and the run time was less than 10 min. The linearity, accuracy, and precision of the method were found to be acceptable over the concentration ranges 6.1–36.4 g mL^–1 for PSE, 65.0–390.0 g mL^–1 for AMP, 3.1–18.6 g mL^–1 for DEX, and 5.0–30.0 g mL^–1 for DPH.     

Tris(2-ethylhexyl)phosphate as an extractant for quadrivalent tin,with subsequent determination with pyrocatechol violet in alloy samples

The solvent extraction of tin(IV) from chloride media withtris(2-ethylhexyl)phosphate is presented. Tin(IV) is extracted quantitatively from 2.75–3.20 mol dm^–3 hydrochloric acid using 6.38–6.91 mol dm^–3 tris(2-ethyl-hexyl)phosphate dissolved in toluene as an extractant. After back-extraction of tin(IV) with water from thetris(2-ethylhexyl)phosphate phase, it is estimated spectrophotometrically following complexation with pyrocatechol violet. The recommended range for determination of tin(IV) is 10–100 g. The probable extracted species is SnCl₄·2TEHP. The method is applicable to the analysis of alloy samples with a detection limit of 0.4 g/ml (for 10 g of tin) and a relative standard deviation between 0.21–0.32%.     

Simultaneous capillary GC-MS determination of triazines and amides in water

Summary A simultaneous capillary Gas Chromatographic-Mass Spectrometric (GC-MS) method is described for the determination of thirteen pesticides belonging to the triazine and amide families in water. The sample is extracted in liquid-liquid mode (dichloromethane) and then the determination of the residues is carried out by capillary gas chromatography with mass spectrometric detection in the Selected-Ion Monitoring mode (SIM). The average recoveries of spiked compounds are in the 78.4–135.4% range between the relative low level (0.100 g L^–1) and the relative high level (10.0 g L^–1). The limits of detection (LOD) are in the 0.009–0.128 g L^–1 range.     

Characterization of airborne particulates by laser microprobe mass analysis

Summary Laser microprobe mass analysis (LAMMA) was applied to characterize aerosol particles collected and separated from 16m to 0.06m by a low pressure cascade impactor. Positive ion LAMMA spectra showed characteristic molecular peaks such as PbCl⁺, a series of Si₂O⁺–Si₂O₄ ⁺ and NaAl₂Si₂O₂ ⁺–NaAl₂Si₂O₅ ⁺, and TiO⁺ in 0.06–0.12m, 0.5–1m and 4–8m fraction, respectively. In the negative ion LAMMA spectra, it was observed that the fragment peaks of sulfate ions were deficient above 2m and those of nitrate ions were deficient under 2m. LAMMA allows remarkable insights into the chemical nature of aerosol particles.

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Charakterisierung luftgetragener Teilchen durch Laser-Microprobe-Massenspektrometrie

Zusammenfassung Laser-Microprobe-Spektrometrie (LAMMS) wurde zur Analyse atmosphärischen Aerosols herangezogen, welches im Korngrößenbereich zwischen 16m und 0.06m mit einem Niederdruckkaskadenimpaktor fraktioniert gesammelt wurde. Positive LAMMS-Spektren zeigten charakteristische molekulare Peaks, wie etwa PbCl⁺, eine Serie von Si₂O⁺–Si₂O₄ ⁺ und NaAl₂Si₂O₂ ⁺–NaAl₂Si₂O₅ ⁺, sowie TiO⁺ in der 0,06–0,12-m,- 0,5–1–m- bzw. 4–8-m-Fraktion. In den negativen LAMMS-Spektren konnten über 2m keine Fragmentpeaks für Sulfationen, unter 2m. keine für Nitrationen beobachtet werden. LAMMS ermöglicht eine bemerkenswerte Einsicht in die chemische Natur von Aerosolteilchen.

     

Flow injection chemiluminescence determination of l-cysteine in amino acid mixture and human urine with the BrO3 −–quinine system

In this paper, a novel flow injection chemiluminescence (CL) determination of l-cysteine is proposed. The method is based on the CL reaction of l-cysteine and KBrO₃ in acidic medium. The CL intensity was greatly enhanced in the presence of quinine. The CL intensity was linear with l-cysteine concentration in the range of 0.2–80 g L^–1, and the detection limit was 0.1 g L^–1 (3). A complete analysis, including sampling and injecting, could be performed in 1 min, giving a throughput of about 60 h^–1. The relative standard deviation was 1.6% for 0.8 g L^–1 l-cysteine (n=11). The proposed method was satisfactorily applied to the determination of cysteine in an amino acid mixture and human urine. The mechanism of the CL reaction is also discussed.     

Development of a stir-bar-sorptive extraction–liquid desorption–large-volume injection capillary gas chromatographic–mass spectrometric method for pyrethroid pesticides in water samples

Stir-bar-sorptive extraction followed by liquid desorption and large-volume injection capillary gas chromatography with mass spectrometric detection (SBSE–LD–LVI-GC–MS), had been applied for the determination of ultra-traces of eight pyrethroid pesticides (acrinathrin, cypermethrin, deltamethrin, esfenvalerate, fenpropathrin, fenvalerate, and permethrin cis and trans isomers) in water samples. Instrumental calibration for selected-ion monitoring acquisition and conditions that could affect the SBSE–LD efficiency are fully discussed. By performing systematic assays on 30-mL water samples spiked at the 0.10 g L^–1 level it was established that stir-bars coated with 47 L polydimethylsiloxane, an equilibrium time of 60 min (750 rpm), 5% methanol as organic modifier, and acetonitrile as back-extraction solvent, provided the best analytical performance to monitor pyrethroid pesticides in water matrices. Good accuracy (81.8–105.0%) and remarkable reproducibility (<11.7%) were obtained, and the experimental recovery data were in good agreement with the theoretical equilibrium described by octanol–water partition coefficients (log K_O/W), with the exception of acrinathrin for which lower yields were measured. Excellent linear dynamic ranges between 25 and 400 ng L^–1 (r²>0.994), low quantification (3.0–7.5 ng L^–1) and detection (1.0–2.5 ng L^–1) limits were also achieved for the eight pyrethroid pesticides studied. The method was successfully used for analysis of tapwater and groundwater matrices spiked at the 0.10 g L^–1, revealing the suitability of the method for determination of pyrethroid pesticides in real samples. The method was shown be reliable and sensitive and a small volume of sample was required to monitor pyrethroids at ultra-trace levels, in compliance with international regulatory directives on water quality.     

Use of a stopped-flow technique for investigation and determination of thiourea and its <Emphasis Type="Italic">N</Emphasis>-methyl derivatives as inducers of the iodine–azide reaction

A stopped-flow technique has been used to investigate the behaviour of 2-thiourea, 1-methyl-2-thiourea, 1,3-dimethyl-2-thiourea, and 1,1,3,3-tetramethyl-2-thiourea in the induced iodine–azide reaction. This technique enables the progress of the reaction to be followed by monitoring the decrease in the absorbance of the iodine–starch complex at 595 nm. The effect of the concentration of the reagents on the rate of the reaction was investigated and a kinetic method for determination of the compounds is proposed. 2-Thiourea, 1-methyl-2-thiourea, and 1,3-dimethyl-2-thiourea can be determined in the range 3–75 mol L^–1 and 1,1,3,3-tetramethyl-2-thiourea in the range 2–200 mol L^–1.     

Determination of hexavalent chromium by using speciated isotope-dilution mass spectrometry after microwave speciated extraction of environmental and other solid materials

Precise and accurate determination of hexavalent chromium in different types of solid environmental sample is regarded as a technical challenge with significant potential error if historically accepted methods are used. Microwave-assisted alkaline extraction (0.5 mol L^–1 NaOH+0.28 mol L^–1 Na₂CO₃) followed by anion-exchange chromatographic separation and inductively coupled plasma mass spectrophotometric detection has been shown to provide accurate and precise results. To obtain a better understanding of potential species conversion during and/or after extraction steps, speciated isotope-dilution mass spectrometry (SIDMS) (EPA Method 6800) metrology has been successfully applied as a diagnostic tool with the modified accompanying extraction version of EPA Method 3060A. In our study, aggregate materials distributed over a large area of a major western US state were found to contain a high concentration of total chromium (195±13 to 709±19 g g^–1) and significant amounts of Cr⁶⁺ (141±6 to 341±29 g g^–1) which are at least three orders of magnitude higher than the US EPA threshold limit (0.5 g g^–1). Sediment samples from a major western US state, studied independently, were found to contain less (1.77±0.34 g g^–1) or no Cr⁶⁺ in the presence of significant total chromium.