Determination of pesticides and PCBs in honey by solid-phase extraction cleanup followed by gas chromatography with electron-capture and nitrogen–phosphorus detection

A multiresidue method for determination of 15 organochlorine pesticides (OCPs), six polychlorinated biphenyls (PCBs), and seven organophosphorus pesticides (OPPs) is implemented for routine determinations of residues in honey. The method involves solid-phase extraction cleanup and determination by GC–ECD/NPD. Quantitation limits ranged from 0.1 to 0.6 g kg^–1 honey for OCPs and PCBs, and from 5.0 to 25.0 g kg^–1 honey for OPPs. Recoveries of OCPs ranged between 77.4 and 94.0%; for PCBs they were from 63.8 to 73.5%. Recovery assays for OPPs varied from 66.7 to 98.1%. The method was applied to the analysis of 111 honey samples from Aragón, Spain. The results obtained indicated a low level of contamination by pesticide residues and PCBs, which can contribute to ensuring the consumer has a safe wholesome supply of honey.     

Matrix Solid-Phase Dispersion Combined with GC–MS/MS for the Determination of Organochlorine Pesticides and Polychlorinated Biphenyls in Marketed Seafood

An analysis method based on matrix solid-phase dispersion (MSPD) and gas chromatography tandem mass spectrometry was developed and applied for the analysis for organochlorine pesticides (OCPs) and polychlorinated biphenyls (PCBs) in the marketed seafood such as fish, shrimp and shellfish. The parameters of the method including the type and amount of the absorbent, as well as the type and volume of the elution solution were optimized. The recoveries were between 70 and 120% with RSDs less than 20%, and the LODs and LOQs were 0.011–0.046 and 0.037–0.153 ng g^?1 under optimized conditions. The results showed that most of the OCPs and PCBs were detectable in the marketed samples with the average concentration range of 0.722–14.206 and 0.034–1.184 ng g^?1, respectively. Among the 21 OCPs detected, DDTs had a relatively higher concentration level. And in the PCBs, the concentration of PCB28 was over 45% of the total PCBs determined in all the samples. The developed method was simple, fast and effective, and could successfully be applied for trace amount of OCPs and PCBs determination in seafood matrixes.     

A Large Volume Injection Procedure for GC-MS Determination of PAHs and PCBs

A simple on-column injection system for large volume of liquid samples for the GC-MS determination of traces of PAHs and PCBs has been investigated. A deactivated fused silica capillary 20 m × 0.53 mm I.D. and 2 meters of an HP5 column (0.53 mm,1 m film thickness) were used as retention gaps. Injection volumes of 80 L for PAHs and 90 L for PCBs, allow determination of 5–50 ng L^–1 PAHs and 11–44 ng L^–1 PCBs in hexane solution with an RSD of < 10%. The method has been used for the determination of PCBs and PAHs in soil sample.     

Determination of microcystins in natural blooms and cyanobacterial strain cultures by matrix solid-phase dispersion and liquid chromatography–mass spectrometry

An analytical procedure based on matrix solid-phase dispersion (MSPD) and liquid chromatography–mass spectrometry (LC-MS) was developed for determining three microcystins (MCs) in natural water blooms and cyanobacteria strain cultures. The procedure involves sample homogenization with C₁₈, washed with dichloromethane to eliminate interfering compounds, and elution with acidic methanol. Results were compared to those achieved by using an organic solvent standard method. Mean recoveries of MCs with MSPD were 85–92% with intra-day relative standard deviation (RSDs) of 9–19%, whereas organic solvent extraction resulted in recovery rates of 92–105% with intra-day RSDs ranging from 8 to 18%. Limits of quantification (LOQs) were 1 g g^–1 dry weight for the MCs either by MSPD or organic solvent extraction. The two analytical methods tested were specific and sensitive to the extraction of MCs and were applied to the detection of MCs in water blooms and culture strains. The concentration of MCs varied from 7 to 3,330 g g^–1 of lyophilized cells with MC-LR always showing the highest concentration. MCs levels were higher in culture strains than in water blooms, except for MC-LR, whose concentration in blooms was slightly superior to that determined in culture strains.     

Matrix Solid-Phase Dispersion Micro-Extraction of Pesticides from Single Insects with Subsequent GC–MS Analysis

A simple multiresidue method based on matrix solid-phase dispersion (MSPD) micro-extraction was studied to determine various organophosphorus (OPPs) and pyrethroid pesticides in single insects. Optimisation of the relevant parameters showed that, in the case of OPPs and permethrin, extraction from 40 mg of isopod (Porcellio scaber) and the use of C₈-bonded silica and 100 L of ethyl acetate were the best conditions, while silica and 3.5 mL of n-hexane were optimal for the less polar pyrethroids. Subsequently, 1 L (ethyl acetate) or 20 L (n-hexane) of the extracts were analysed by GC–MS without any further clean-up. The limits of detection (LODs), in the SIM mode, were 5–80 ng g^–1 for most OPPs and trans-permethrin (cis-permethrin 0.3 ng g^–1) when using the C₈-bonded silica/ethyl acetate procedure, and 5–35 ng g^–1 for the pyrethroids when using the silica/n-hexane procedure. The recoveries of the OPPs and pyrethroids from the isopods were 52–94%. The practicality of the proposed method was studied for pesticides in isopods which had been fed polluted leaves.     

Three new mussel tissue standard reference materials (SRMs) for the determination of organic contaminants

Three new mussel tissue standard reference materials (SRMs) have been developed by the National Institute of Standards and Technology (NIST) for the determination of the concentrations of organic contaminants. The most recently prepared material, SRM 1974b, is a fresh frozen tissue homogenate prepared from mussels (Mytilus edulis) collected in Boston Harbor, Massachusetts. The other two materials, SRMs 2977 and 2978, are freeze-dried tissue homogenates prepared from mussels collected in Guanabara Bay, Brazil and Raritan Bay, New Jersey, respectively. All three new mussel tissue SRMs complement the current suite of marine natural-matrix SRMs available from NIST that are characterized for a wide range of contaminants (organic and inorganic). SRM 1974b has been developed to replace its predecessor SRM 1974a, Organics in Mussel Tissue, for which the supply is depleted. Similarly, SRMs 2977 and 2978 were developed to replace a previously available (supply depleted) freeze-dried version of SRM 1974a, SRM 2974, Organics in Freeze-Dried Mussel Tissue. SRM 1974b is the third in a series of fresh frozen mussel tissue homogenate SRMs prepared from mussels collected in Boston Harbor starting in 1988. SRM 1974b has certified concentration values for 22 polycyclic aromatic hydrocarbons (PAHs), 31 polychlorinated biphenyl congeners (PCBs), and 7 chlorinated pesticides. Reference values are provided for additional constituents: 16 PAHs, 8 PCBs plus total PCBs, 6 pesticides, total extractable organics, methylmercury, and 11 trace elements. PAH concentrations range from about 2 ng g^–1 dry mass (cyclopenta[cd]pyrene) to 180 ng g^–1 dry mass (pyrene). PCB concentrations range from about 2 ng g^–1 dry mass (PCB 157) to 120 ng g^–1 dry mass (PCB 153). The reference value for total PCBs in SRM 1974b is (2020 ± 420) ng g^–1 dry mass. Pesticide concentrations range from about 4 ng g^–1 dry mass (4,4-DDT) to 40 ng g^–1 dry mass (4,4-DDE). SRM 2977 has certified values for 14 PAHs, 25 PCB congeners, 7 pesticides, 6 trace elements, and methylmercury. Reference values for 16 additional PAHs and 9 inorganic constituents are provided, and information values are given for 23 additional trace elements. SRM 2978 has certified and reference concentrations for 41 and 22 organic compounds, respectively, and contains contaminant levels similar to those of SRM 1974b. Organic contaminant levels in SRM 2977 (mussels from Guanabara Bay, Brazil) are typically a factor of 2 to 4 lower than those in SRM 1974b and SRM 2978. The organic contaminant concentrations in each new mussel tissue SRM are presented and compared in this paper. In addition, a chronological review of contaminant concentrations associated with mussels collected in Boston Harbor is discussed as well as a stability assessment of SRM 1974a.Electronic Supplementary Material Supplementary material is available in the online version of this article at . A link in the frame on the left on that page takes you directly to the supplementary material.     

Spectrophotometric determination of microamounts of thorium with disodium salt of 2-(2-hydroxy-3,6-disulfo-1-naphthylazo)-benzenearsonic acid (Thorin) as a chromogenic reagent

A sensitive spectrophotometric method has been developed for the determination of microamounts of thorium using 0.05% thorin in a 3M perchloric acid solution as a chromogenic reagent and measuring the absorbance at 544 nm. The complex of thorium thus formed, is stable for more than two months with a constant absorbance of ±0.55%. Beer's law is obeyed from 0 to 25 g g^–1 of thorium in a solution with a molar absorptivity (544 nm) = 1.69×10⁴ M^–1 cm^–1 at 26±1 °C. Among the anions tested, only phosphate, acetate and cyanide at >200-fold excess of thorium interfere in the determination, whereas cations like Zn(II), Al(III), Na(I), Mg(II), and Ca(II) do not effect the absorbance. Thorium can be determined in the presence of oxalate, nitrate, tartrate, sulfate, thiosulfate, citrate, and ascorbate. The accuracy of the method has been checked by measuring the known concentration of thorium in the range of 100 g-5 mg g^–1 and found to be in the range of 7.7–0.9%. The method has been applied successfully to determine thorium at g g^–1 level in local ore samples with a precision of ±0.3%. The sensitivity of the method on Sandell's scale is 0.082±0.002 g g^–1 cm^–1.     

Matrix Solid Phase Dispersion‐Accelerated Solvent Extraction for Determination of OCP Residues in Fish Muscles

A rapid, sensitive and accurate matrix solid phase dispersion‐accelerated solvent extraction (MSPD‐ASE) method for selective determination of sixteen organochlorine pesticide (OCP) residues in fish samples has been developed and validated. 2 g fresh fish muscle was dispersed with 10 g anhydrous sodium sulfate and 2 g acid alumina thoroughly, and loaded into the stainless‐steel extraction cell containing 6 g of acid alumina and 10 g anhydrous sodium sulfate. The temperature 60 °C and two extraction cycles of 5 min gave adequate extraction efficiency using DCM‐hexane (3:7, v/v) mixture as solvent. Not only the lipids, but also other co‐extracts, which peaks mostly located in the forepart of chromatograms and maybe interfere the identification or quantitation of analytes, were eliminated exhaustively, while analytes were extracted selectively. Sixteen OCPs were identified by retention time of standards and quantified using mirex as internal standards. These detected OCPs were confirmed by GC‐MS in real samples. The performance of proposed method was evaluated and validated: the detection limits were 0.008‐0.05 ng g^‐1, relative standard deviations were 1.9‐5.0%, and recoveries were 91.0‐104.1% spiked at 10 ng g^‐1 level. The accuracy and precision of proposed method were equal to or better than that of traditional Soxhlet extraction method.     

A toxic reagent-free method for normal-phase matrix solid-phase dispersion extraction and reversed-phase liquid chromatographic determination of aldrin,dieldrin, and DDTs in animal fats

A method for the determination of aldrin, dieldrin, DDT, DDE, and DDD contamination in animal fats (beef tallow, lard, and chicken fat) without using toxic reagents is developed, that uses high-performance liquid chromatography after the sample has been prepared by matrix solid-phase dispersion (MSPD) with acidic alumina oxide. A reversed-phase C₁-silica column with a mobile phase of 50% (v/v) ethanol solution (in water) and a photo-diode array detector were used for the determination. Average recoveries of the target compounds (0.2–5.0 g g^–1) ranged from 84–98%, with coefficients of variation of <5%. The limits of quantitation were 0.16 g g^–1 for AD, 0.10 g g^–1 for DD, 0.06 g g^–1 for DDT, 0.07 g g^–1 for DDE, and 0.05 g g^–1 for DDD. No toxic reagents were used at all.     

Assessment of the essential element and heavy metal content of edible fish muscle

The aim of this work was to determine the concentrations of some essential and toxic elements in the muscle of ten species of commercial fish consumed in Portugal. We combined two different techniques for determination of the elements—energy-dispersive X-ray fluorescence (EDXRF) was used to quantify K, Ca, Fe, Zn, Se, Rb, and Sr and flame atomic-absorption spectrometry for analysis of Cr, Ni, Cu, Cd, Hg, and Pb. The latter technique was used because of its higher sensitivity, because these elements were not detected by EDXRF. The results obtained show a similar pattern for the trace elements. K and Ca are present at the highest concentrations in all the samples studied, from 0.6–1.3% and from 0.04–0.08%, respectively, followed by Zn, Fe, Sr, Se, and Rb. Sr is present at higher concentrations than Rb in all the species studied except meagre. Concentrations of the elements in octopus do not follow this pattern—Fe is present at a higher concentration than Zn. Low concentrations of Cr (0.66–1.5 g g^–1), Ni (0.11–0.24 g g^–1), Cd (0.01–0.08 g g^–1), Hg (0.49–2.74 g g^–1), and Pb (0.02–0.06 g g^–1) were observed in all the samples analysed. The concentration of Hg was highest in Helicolenus dactylopterus—5.4 g g^–1 in one sample.     

Determination of lead in bone tissues by axially viewed inductively coupled plasma multichannel-based emission spectrometry

A new procedure for determining low levels of lead in bone tissues has been developed. After wet acid digestion in a pressurized microwave-heated system, the solution was analyzed by inductively coupled plasma multichannel-based emission spectrometry. Internal standardization using the Co 228.615 nm reference line was chosen as the optimal method to compensate for the matrix effects from the presence of calcium and nitric acid at high concentration levels. The detection limit of the procedure was 0.11 g Pb g^–1 dry mass. Instrumental precision at the analytical concentration of ~10 g l^–1 ranged from 6.1 to 9.4%. Precision of the sample preparation step was 5.4%. The concentration of lead in SRM 1486 (1.32±0.04 g g^–1) found using the new procedure was in excellent agreement with the certified level (1.335±0.014 g g^–1). Finally, the method was applied to determine the lead in various fish bone tissues, and the analytical results were found to be in good agreement with those obtained through differential pulse anodic stripping voltammetry. The method is therefore suitable for the reliable determination of lead at concentration levels of below 1 g g^–1 in bone samples. Moreover, the multi-element capability of the technique allows us to simultaneously determine other major or trace elements in order to investigate inter-element correlation and to compute enrichment factors, making the proposed procedure particularly useful for investigating lead occurrence and pathways in fish bone tissues in order to find suitable biomarkers for the Antarctic marine environment.     

An SPME–GC–MS Method for Determination of Organochlorine Pesticide Residues in Medicinal Plant Infusions

A simple method, direct-immersion sampling by solid-phase microextraction and gas chromatography–mass spectrometry (DI-SPME–GC–MS), has been developed for determination of organochlorine pesticides (OCP) in plant infusions. The optimum conditions for SPME with a 100-m PDMS-coated fiber were established by using a central composite design. The extraction time and sample temperature established were 60 min and 50 °C, respectively. The method was validated and used to determine hexachlorobenzene, lindane, 4,4-DDE, aldrin, dieldrin, endrin, heptachlor, heptachlor epoxide, and 4,4-DDT in infusions of Mikania laevigata and Maytenus ilicifolia. Limits for quantitation for the OCP were between 0.2 and 2.0 ng g^–1 except for lindane, for which the LOQ was higher (12 ng g^–1), because of its low affinity for the PDMS fiber. Recovery was in the range 90 to 108% and the intra-assay precision was below 17%. Transfer of the OCP from the plant to the infusion was in the range 0.34 to 3.4% and was correlated with the solubility of each compound in water.     

Determination of prostatic androgens in 10 mg of tissue using liquid chromatography–tandem mass spectrometry with charged derivatization

A practical liquid chromatography–tandem mass spectrometric (LC-MS-MS) method for the determination of prostatic 5-dihydrotestosterone (DHT) and testosterone (T) has been developed. The prostatic androgens were extracted with MeOH–H₂O (3: 7, v/v), purified with an Oasis HLB cartridge, derivatized with the permanently charged reagent 2-hydrazino-1-methylpyridine (HMP), and subjected to LC–MS-MS analysis using electrospray ionization (ESI) operated in the positive ion mode. The derivatization with HMP was very effective at increasing the detectability using the positive-ESI-MS. The method allowed the reproducible and accurate quantification of ng g^–1 tissue levels of prostatic androgens in 10 mg of tissue. That is, the intra- and inter-assay coefficients of variation were below 8.1 and 9.3%, respectively, and the analytical recoveries of the androgens were quantitative. The limits of quantitation for DHT and T were both 1.0 ng g^–1 tissue. The developed method was used to determine DHT and T in the prostates of patients with benign prostatic hyperplasia and prostate cancer, and satisfactory results were obtained.     

New method based on combining ultrasonic assisted miniaturized matrix solid-phase dispersion and homogeneous liquid-liquid extraction for the determination of some organochlorinated pesticides in fish

In this study, ultrasonic assisted miniaturized matrix solid-phase dispersion (US-MMSPD) combined with homogeneous liquid–liquid extraction (HLLE) has been developed as a new method for the extraction of organochlorinated pesticides (OCPs) in fish prior to gas chromatography with electron capture detector (GC-ECD). In the proposed method, OCPs (heptachlor, aldrin, DDE, DDD, lindane and endrin) were first extracted from fish sample into acetonitrile by US-MMSPD procedure, and the extract was then used as consolute solvent in HLLE process. Optimal condition for US-MMSPD step was as follows: volume of acetonitrile, 1.5 mL; temperature of ultrasound, 40 °C; time of ultrasound, 10 min. For HLLE step, optimal results were obtained at the following conditions: volume of chloroform, 35 μL; volume of aqueous phase, 1.5 mL; volume of double distilled water, 0.5 mL; time of centrifuge, 10 min. Under the optimum conditions, the enrichment factors for the studied compounds were obtained in the range of 185–240, and the overall recoveries were ranged from 39.1% to 81.5%. The limits of detection were 0.4–1.2 ng g⁻¹ and the relative standard deviations for 20 ng g⁻¹ of the OCPs, varied from 3.2% to 8% (n = 4). Finally, the proposed method has been successfully applied to the analysis of the OCPs in real fish sample, and satisfactory results were obtained.     

Spectrophotometric Determination of Thorium with Disodium Salt of Arsenazo-III in Perchloric Acid

A rapid and sensitive spectrophotometric method has been developed for the determination of thorium using 0.04% Arsenazo-III in a 2M perchloric acid solution. Absorbance was measured in 1 cm cell and the complex has a sensitive absorption peak at 654 nm. The complex is formed instantly in perchloric acid and remains stable for 45 minutes with constant absorbance. Beer's law is obeyed in the range 1–60 g·g^–1 of thorium concentration with a molar absorptivity at 654 nm = 3.07·10⁵ M^–1·cm^–1 at 24±2°C. The foreign ions interference in thorium determination have been checked. The cations were tested at >60-fold excess of thorium, Mn(II), Fe(III), Co(II) and Ni(II) interfere negatively, whereas only Ce(III) has increased the absorbance. Among the anions, cyanide, phosphate, thiocyanate and acetate at 150-fold excess of thorium cause significant interference. However, thorium can bedetermined in the presence of nitrate, chloride, oxalate, tartrate, ascorbate, thiosulphate and citrate. The method has been applied on certified reference material for thorium determination after extractive separation and the result was found in good agreement with the certified value. The method has been also applied successfully to determine thorium at g·g^–1 level in local ore samples with a precision of ±0.04%.     

Determination of inorganic arsenic in white fish using microwave-assisted alkaline alcoholic sample dissolution and HPLC-ICP-MS

An analytical method for the determination of inorganic arsenic in fish samples using HPLC-ICP-MS has been developed. The fresh homogenised sample was subjected to microwave-assisted dissolution by sodium hydroxide in ethanol, which dissolved the sample and quantitatively oxidised arsenite (As(III)) to arsenate (As(V)). This allowed for the determination of inorganic arsenic as a single species, i.e. As(V), by anion-exchange HPLC-ICP-MS. The completeness of the oxidation was verified by recovery of As(V) which was added to the samples as As(III) prior to the dissolution procedure. The full recovery of As(V) at 104±7% (n=5) indicated good analytical accuracy. The uncertified inorganic arsenic content in the certified reference material TORT-2 was 0.186±0.014 ng g^–1 (n=6). The method was employed for the determination of total arsenic and inorganic arsenic in 60 fish samples including salmon from fresh and saline waters and in plaice. The majority of the results for inorganic arsenic were lower than the LOD of 3 ng g^–1, which corresponded to less than one per thousand of the total arsenic content in the fish samples. For mackerel, however, the recovery of As(III) was incomplete and the method was not suited for this fat-rich fish.     

Optimization of matrix solid-phase dispersion conditions for UV filters determination in biota samples

A low solvent consumption method for the determination of eight ultraviolet (UV) filters, displaying low to medium polarities, in freeze-dried samples of marine bivalves and fish is proposed. Matrix solid-phase dispersion (MSPD) and gas chromatography with mass spectrometry (GC-MS) were used as sample preparation and determination techniques, respectively. This work describes the influence of several parameters (type and amount of dispersant and clean-up sorbents, as well as elution solvent) on the yield and the selectivity of the MSPD extraction. Under optimized conditions, samples (0.5?g) were ground with 2?g of Florisil in a mortar with a pestle and transferred into a polypropylene syringe, which contained 1?g of C18 as clean-up sorbent. Analytes were eluted with 5?mL of acetonitrile. This extract was concentrated to dryness, re-constituted with 1?mL of ethyl acetate and injected in the GC-MS system without any further clean-up. The global average recoveries, measured for three different biota samples, spiked at three different levels (between 50 and 1000?ng?g^?1), ranged from 80% to 101% with associated standard deviations below 10%. The inter-day precision of the method varied from 4% to 15% and the achieved LOQs (defined for a signal to noise ratio of 10) ranged from 4 to 28?ng?g^?1, referred to the freeze-dried matrix. Octocrylene (OCR) was found in some samples of fish and mussels at concentrations between 15 and 20?ng?g^?1, referred to dry mass.     

Occurrence of organochlorine pesticides and polychlorinated biphenyls in soils and sediments from Eastern Romania

Polychlorinated biphenyls (PCBs) and organochlorine pesticides (OCPs), such as DDT and analogues, hexachlorocyclohexane (HCH) isomers and hexachlorobenzene (HCB), were measured in surface soils and sediments from Eastern Romania. Thirty-nine soil samples from the forested zone, eight soil samples from a municipal waste-disposal site, and 10 sediment samples from the Bahlui River along the Iassy city were analysed using accelerated solvent extraction (ASE) and gas chromatography coupled to electron capture detection or mass spectrometry. The low mean concentrations of OCPs (11–31 and 22–84?ng?g^?1 for HCHs and DDTs, respectively) and PCBs (8–43?ng?g^?1) in soil samples from the forested zone suggest that contamination at most of these sites occurred predominantly through atmospheric transport from zones where these compounds were used and subsequently through atmospheric deposition. Contrarily, soil samples collected in the vicinity of a waste-disposal site near Iassy contained higher mean levels of PCBs (278?ng?g^?1, range 34–1132?ng?g^?1) than OCPs (6 and 101?ng?g^?1 of soil for HCHs and DDTs, respectively). The sediment samples collected along the Bahlui river throughout the Iassy city revealed higher mean levels of PCBs (59?ng?g^?1, range 24–158?ng?g^?1) compared with OCP levels (2 and 37?ng?g^?1 of soil for HCHs and DDTs, respectively). Furthermore, PCB profiles and concentrations in the sediment samples varied considerably along the river due to a wide variety of sources, such as different industries and waste sites. Although their sources are difficult to evaluate, the presence of POPs at most sites (especially at the waste-disposal site) may constitute a potential health hazard.     

Sensitive Method for Trace Determination of Mercury in Wines Using Electrothermal Atomic Absorption Spectrometry

An accurate, simple and precise method for total mercury determination in wines is described. Liquid/liquid extraction of inorganic and organic mercury species directly from untreated wine samples is recommended as a preconcentration procedure prior to determination by electrothermal atomic absorption spectrometry (ETAAS). Ammonium pyrrolidinedithiocarbamate was used as complexation agent. The optimal instrumental parameters for ETAAS measurement of mercury species extracted are proposed. The detection limit for total mercury determination is 0.2µgL^–1. The relative standard deviation is 15–22% for mercury in wine in the range of 0.2–5µgL^–1. The proposed procedure has been successfully applied to the determination of mercury in bottled wines in Bulgaria and Macedonia.     

Trace determination of some phenolic growth-promoting hormones in meat by high-performance liquid chromatography with voltammetric detection

Summary The oxidative voltammetric behaviour of the growth-promoting hormones oestriol, 17-oestradiol, oestrone, diethylstilboestrol, dienoestrol and hexoestrol has been investigated at the glassy carbon electrode. The voltammetric responses obtained for these compounds in acid media were found to be the most suitable for analytical purposes. Based on this study, a sensitive, rapid and convenient method has been developed for their determination by high-performance liquid chromatography utilising voltammetric detection. This method could determine oestrone and hexoestrol down to 1–2 ng g^–1 and 17-oestradiol, diethylstilboestrol and dienoestrol down to 2–3 ng g^–1 in meat, but was unable to determine oestriol at this level due to the presence of co-extracted interferences.

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Spurenbestimmung einiger phenolischer wachstumsfördernder Hormone in Fleisch durch HPLC mit voltammetrischer Detektion

Zusammenfassung Das oxidative voltammetrische Verhalten der wachstumsfördernden Hormone Östriol, 17-Östradiol, Östron, Diethylstilböstrol, Dienöstrol und Hexöstrol wurde an der glasigen Kohlenstoffelektrode untersucht und als für analytische Zwecke sehr geeignet befunden. Ein schnelles und empfindliches Verfahren wurde ausgearbeitet, das auf HPLC-Trennung mit voltammetrischer Detektion beruht. Östron und Hexöstrol können bis herab zu 1–2 ng g^–1 und 17 -Östradiol, Diethylstilböstrol sowie Dienöstrol bis zu 2–3 ng g^–1 in Fleisch erfaßt werden. Östriol kann jedoch in diesem Konzentrationsbereich nicht bestimmt werden, da mitextrahierte Substanzen stören.