Multiresidue method for the gas chromatographic determination of pesticides in honey after solid-phase extraction cleanup

A new multiresidue method is described for the determination of pesticides in honey. The method involves dissolution of the honey in a methanol-water mixture, followed by solid-phase extraction cleanup and gas chromatographic determination. Twenty-six pesticides used on flowering field crops, on flowering fruit and vegetables, or as acaricides to control Varroa jacobsoni in beehives are determined by the method. Recoveries from honey, spiked at 0.02-1.6 mg/kg, ranged from 85 to 127% with a relative standard deviation (RSD) of 2-16%, except for the RSD of 27% for captan at 0.05 mg/kg.     

Continuous solid-phase extraction and gas chromatographic determination of organophosphorus pesticides in natural and drinking waters

A simple, rapid continuous-flow solid-phase extraction method with gas chromatographic detection for the determination of organophosphorus pesticides is proposed. The continuous system consists of an adsorbent column where pesticides are preconcentrated and subsequently eluted with ethyl acetate. Various sorbent materials were assayed of which RP-C18 was found to provide the best results, with a sorption efficiency close to 100%. A comparative study of the determination of pesticides in aqueous samples was conducted using gas chromatography with nitrogen-phosphorus (NPD) and flame ionization (FID) detection. The detection limits of the method for 10 ml of sample were between 50-130 ng/l and 4.5-1 1.7 microg/l with NPD and FID detection, respectively. The method was used to determine organophosphorus pesticides in river, pond, well and tap waters, all with good precision (2.9-4.3%) and recoveries ranging from 93.8 to 104.5%.     

Multiwalled carbon nanotubes as solid-phase extraction materials for the gas chromatographic determination of organophosphorus pesticides in waters

In the present work, a GC method with nitrogen-phosphorus detection (NPD) was developed for the simultaneous determination of eight organophosphorus pesticide (OPP) residues (i.e., ethoprofos, diazinon, chlorpyrifos-methyl, fenitrothion, malathion, chlorpyrifos, fenamiphos, and buprofezin) in water samples. Preconcentration of the water samples was carried out using an SPE procedure with multiwalled carbon nanotubes (MWCNTs) of 10-15 nm od, 2-6 nm id, and 0.1-10 microm length as stationary phase. Extraction parameters, such as the amount of MWCNTs, sample volume, pH, and type and amount of the eluent were optimized. The most favorable conditions were as follows: 40 mg MWCNTs, 800 mL water, pH 6.0, and 20 mL dichloromethane, respectively. The MWCNTs-SPE-GC-NPD method was applied to the determination of these pesticides in real water samples: mineral and ground water as well as run-off water from an agricultural area collected shortly before opening out onto the sea. A recovery study was developed with five consecutive extractions of the three types of water spiked at three concentration levels (n = 15). Mean recovery values were in the range of 75-116% for mineral water (RSD < 6.3%), 67-119% for ground water (RSD < 5.8%), and 57-81% for run-off waters (RSDs < 6.9%), except for fenamiphos (mean recovery values between 40 and 84% for the three types of waters, RSDs < 8.9%). LODs were in the low ng/L level (i.e., levels below the maximum residue limits (MRLs) established by the European Union (EU) legislation for these compounds in waters). The proposed method was also applied to the analysis of six water samples (two of each type: mineral, ground, and run-off waters) in which no residues of the selected pesticides were found. Results show that the MWCNTs used in this work have a high adsorbability of the pesticides under study. The main advantage of the use of these MWCNTs is their low cost when compared with those MWCNTs previously used in the literature and with conventional SPE cartridges.     

Extraction, quantitative gas chromatographic determination and gas chromatographic/mass spectrometric detection of ecgonine for identification of cocaine and its metabolites in urine

Summary Quantitative extraction studies from urine were carried out by addition of cocaine, benzoylecgonine, ecgonine methyl ester and ecgonine to urine samples. After hydrolysis to ecgonine the compounds were analyzed together. Ecgonine was isolated by a cation-exchange resin and purified by an anion-exchange resin. The quantitative determination was performed by GC after silylation with MSTFA. The recovery was 77% at a concentration of 150 g ecgonine/ml urine. A qualitative determination of ecgonine by GC/MS was possible up to the detection limit of 20 ng/ ml. The method can be applied for the detection of cocaine abuse.

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Extraktion, quantitative gas-chromatographische Bestimmung und gas-chromatographischer massenspektrometrischer Nachweis von Ecgonin zur Identifizierung von Cocain und seinen Metaboliten in Urin

Zusammenfassung Es wurden quantitative Untersuchungen zur Extraktion von Urin durchgeführt, dem Cocain, Benzoylecgonin, Ecgoninmethylester und Ecgonin zugesetzt wurden. Die Summe dieser Verbindungen kann über eine vorgeschaltete Hydrolyse zu Ecgonin indirekt bestimmt werden. Nach Hydrolyse wird Ecgonin an einem Kationenaustauscher isoliert und der Extrakt an einem Anionenaustauscher gereinigt. Die quantitative Bestimmung erfolgt gaschromatographisch nach Silylierung mit MSTFA. Dabei beträgt die Wiederfindungsrate 77% bei Konzentrationen von 150 g Ecgonin/ml Urin. Der qualitative Nachweis von Ecgonin durch GC/MS ist bis zu einer Nachweisgrenze von 20 ng/ml möglich. Damit eignet sich die Methode zum Nachweis einer Cocain-Einnahme im Urin.

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From the dissertation by U. Zerell, University of Bonn, 1986 (in preparation)     

Evaluation of analyte protectants to improve gas chromatographic analysis of pesticides

A common problem in gas chromatography (GC) applications is the analyte losses and/or peak tailing due to undesired interactions with active sites in the inlet and column. Analytes that give poor peak shapes or degrade have higher detection limits, are more difficult to identify and integrate, and are more prone to interferences than stable analytes that give narrow peaks. For susceptible analytes, significant peak quality improvements are obtained when matrix components are present because they fill active sites, thus reducing analyte interactions. This phenomenon is called "matrix-induced chromatographic response enhancement." Several approaches have been proposed to minimize peak distortion phenomena and compensate for matrix-induced effects, which is especially important for accurate quantitation, but each approach has serious limitations for routine multi-pesticide analysis. In this study, we demonstrate the feasibility of using "analyte protectants" to provide a more convenient and effective solution to the problem than other approaches developed thus far. The protecting agents are added to extracts and matrix-free standards alike to provide the chromatographic enhancement effect even for the most susceptible analytes in a very dirty GC system. In this study, we evaluated 93 different compounds to find the most suitable ones for improving chromatographic quality of the signal. Because hydrogen bonding has been shown to be an important factor in analyte interactions with active sites, we mainly focused on additives with strong hydrogen bonding capabilities. Dramatic peak enhancements were achieved using compounds containing multiple hydroxy groups, such as sugars and sugar derivatives, and gulonolactone appears to be the most effective protecting agent for the most pesticides that we tested. The benefits of using analyte protectants versus alternative procedures for overcoming matrix-induced effects in quantitation include: (a) simpler procedure; (b) easier integration of peaks; (c) lower detection limits; (d) better quantitation; (e) less maintenance of the GC inlet; and (e) lower cost. However, long-term influences on the performance of the chromatographic system have yet to be established.     

Characterisation of wax works of art by gas chromatographic procedures

To identify the various natural and synthetic substances used by sculptors at the end of the 19th century, several contemporary reference samples were investigated by high temperature gas chromatography (HT GC) and HT GC-MS. Using specific chromatographic conditions and minimising sample preparation, we could separate, detect and identify a wide range of biomolecular markers covering a great variety of molecular weights and volatilities, with a minimum amount of sample, in a single run. Beeswax, spermaceti, carnauba, candellila and Japan waxes as well as pine resin derivatives, animal fats, paraffin, ozokerite and stearin, used as additives in wax works of art, were chemically investigated. In the case of low volatile compounds, transbutylation was performed. The structure of long-chain esters of spermaceti was elucidated for the first time by HT GC-MS analysis. Such a method was then carried out on 10 samples collected on a statuette of Junon by Antoine-Louis Barye (Louvre Museum, Paris, France) and on a sculpture by Aimé-Jules Dalou (Musée de la Révolution Fran?aise, Vizille, France). The analytical results obtained provide new data on the complex recipes elaborated by sculptors at the end of the 19th century.     

Headspace gas chromatographic determination of ethylene oxide in air

Summary A simple and accurate headspace-GC method is described to determine the amount of ethylene oxide which has been collected from air using adsorption tubes containing activated charcoal and a relatively safe desorbing agent (N,N-dimethyl acetamide). The detection limit is 40μg/m³.     

Multiresidue procedures for determination of triazine and organophosphorus pesticides in water by use of large-volume PTV injection in gas chromatography

Summary Two procedures, based on large-volume injection with a programmed-temperature vaporizer (PTV), have been developed for the determination of several triazine and organophosphorus pesticides. The use of PTV for injection in gas chromatography (GC) has enabled the introduction of up to 200 μL sample extract into the GC, thus increasing the sensitivity of the method. PTV injection has been combined off-line with two different microextraction procedures—liquid-liquid partition and solid-phase extraction. A simple and rapid off-line liquid-liquid microextraction procedure (5 mL water/1 mL methyltert-butyl ether) was applied to surface water samples spiked at levels between 0.01 and 5μg L⁻¹. Recoveries of the overall procedure were >80% and the precision was better than 15%. Detection limits were <30 ngL⁻¹ from 200-μL injections in GC-NPD analysis of triazines and GC-FPD analysis of organophosphorus pesticides. Off-line automated solid-phase extraction with C₁₈ cartridges has been applied to water samples (50 mL) spiked at 0.01, 0.1 and 1 μg L⁻¹. The overall procedure was satisfactory (recoveries >80% and coefficients of variation <12%) and the limits of detection ranged from 1 to 9 ng L⁻¹. Finally, several surface water samples were anlysed, and triazine herbicides were detected at concentrations of approx. 0.1–0.2 μg L⁻¹. The results were similar to those obtained by conventional solvent extraction then GC-MSD after splitless injection of 2 μL.     

Quick gas chromatographic method for determining common pesticides in musts and wines

Summary A rapid method based on gas chromatography which determines parathion-methyl, fenitrothion, chlorpyrifos, dichlofluanid, vinclozolin, chlozolinate, procymidone and iprodione is described. It involves quantitative extraction with n-hexane and determination by capillary gas chromatography using an electron capture detector. Pesticides were satisfactorily separated in 15 min with a phenylmethylsilicone fused-silica capillary column under isothermal conditions. Quantitation was carried out using dieldrin as internal standard. The method seems appropriate for oenological laboratory work because of its simplicity and rapidity. It was successfully used to identify and quantify pesticides studied in musts and wines.     

Extraction and gas chromatographic determination of methyl-, ethyl-, and methoxyethylmercury(II) halides

The separation, identification, and determination of methyl-, ethyl-, and methoxyethylmercury(II) halides in biological materials were studied. The procedure developed involved a 24-h leach with 1 M sodium iodide, equilibration of the aqueous phase for 2 min with an equal volume of benzene, and then injection of an aliquot of the benzene phase onto a gas Chromatographic column consisting of 5% cyclohexanedimethanol succinate held on Anakrom ABS. Excellent baseline separation of the Chromatographic peaks was obtained. The extraction steps were monitored with RHgX compounds tagged with ²⁰³Hg. Partition coefficients are reported for methyl- and ethylmercury(II) chlorides, bromides, and iodides; several overall formation constants of the anionic complexes RHgCl_n^1-n (n=2, 3) were determined. Results are reported for the recovery of methyl- and ethylmercury(II) halides from inoculated rye seed, humic and inorganic sediment, and fish grown in an aquarium.     

A new gas chromatographic retention index for pesticides and related compounds

A new gas chromatographic (GC) retention index based on a homologous series of tri-n-alkylamines is proposed for use in the detection of pesticides and related compounds because the standard n-paraffin hydrocarbons used for the Kovats index do not show up well on the nitrogen-phosphorus detectors commonly used in pesticide analysis. Using fused silica bonded phase capillary columns (DB-1 or DB-5), the trialkylamine indices of 106 selected pesticides and related compounds were measured and their relationship to the Kovats index determined.     

Solid-phase sample preparation method for prostaglandins: integration of procedures for isolation and derivatization for gas chromatographic determination

A procedure using a solid-phase support has been developed for the isolation and derivatization of prostaglandins from biological matrices. The styrene-divinylbenzene cross-linked copolymeric macroreticular resin, XAD-2, was used as an adsorbent for prostaglandin E2 from biological samples, as a support for the oximation of the carbonyl group and as a catalyst for pentafluorobenzylation. The reactor bed was then linked to a Florisil column for a final chromatographic clean-up. Matrix effects were found to affect the yield, but recovery of the desired electrophoric products was comparable with methods reported in the literature. The ease of sample preparation suggests that this technique may be a viable approach to automating the processes for preparing prostaglandins from biological matrices for gas chromatographic analysis.