Analytical approach for routine methylmercury determination in seafood using gas chromatography-atomic fluorescence spectrometry

Two methodologies have been developed for the analysis of mercury species in seafood by capillary gas chromatography coupled to an AFS detector via pyrolysis. The first one is based on the ethylation of both, inorganic and methylmercury species (Method 1), in which clean-up is not necessary because a small amount of sample is required. In the second one, monoalkylated mercury species are extracted into organic phases after forming the corresponding chlorides (Method 2). In this case the elimination of the interfering compounds from the matrix requires a clean-up step, which enables the treatment of higher quantities of sample. Both procedures can be considered complementary because the concentration range applicable for each one of them is different: 0.75-10 μg_Hg g⁻¹, in dry basis for methylmercury (Method 1) and 6-1000 ng_Hg g⁻¹ (Method 2). The range of application for natural samples can be easily selected by a preliminary analysis of total mercury, because most mercury in seafood is present as MeHg. Optimum parameters for both procedures have been evaluated, and the methods were validated with two standard reference materials (BCR-463 and NIST-2977). Finally, the methods have been applied to the analysis of seafood samples. Detection limits of MeHg range from 1.7 to 220 ng_Hg g⁻¹ (dry basis) depending of the methodology selected and the weight of sample. The method can be successfully applied to commercially available seafood samples, and considered for routine analysis.     

Comparative studies of methylmercury determination in biological and environmental samples

Some parameters affecting the accuracy of various approaches to methylmercury (MeHg) determination in biological and environmental samples were studied. Different isolation techniques (ion-exchange, extraction, volatilization, distillation) and final measurement via cold vapour atomic absorption spectroscopy (CV AA) or gas chromatography (GC) were compared. Results obtained by the various isolation techniques are comparable for almost all biological and environmental samples, except for soils and some sediments, where disagreement between the results obtained by GC and CV AA was found. In order to resolve these problems, a new separation technique based on distillation of MeHg from the sample followed either by CV AA or GC was developed. The new method results in very good recovery and reproducibility (95 ± 2%) for all samples examined (fish, mussel, shrimp, blood, hair, algae, sediment, etc.), is specific for MeHg and provides for its differentiation from other species by an indirect CV AA determination. Gas-chromatographic measurement of the isolated MeHg using different packings and conditioning of the columns is also discussed. The distillation method with GC detection is advantageous in producing cleaner chromatograms and in prolonging the life-time of the packing and the intervals between reconditioning.     

Multicommutation cold vapour atomic fluorescence determination of Hg in water

A multicommutation-based method has been developed for the on-line direct atomic fluorescence spectrometric (AFS) determination of Hg in waters without any previous sample treatment. The performance of the proposed procedure has been compared with that of a conventional AFS system based on continuous mode measurements. In short, the use of multicommutation, together with a reduction of the size of the liquid-gas phase separator, provides an increase of the laboratory productivity by improving the sample throughput by a factor of 3.6 and strongly reduces the sample consumed by a factor of 6 and reagent consumed by a factor of 8.4. The waste generation is reduced by a factor of 2.4 and the Ar consumed by a factor of 6, thus the developed method is an environmentally and economically sustainable alternative to the methodology based on continuous measurements, without any reduction of the analytical sensitivity and with an enhancement of the repeatability of measurements. Only the limit of detection was poorer for the methodology developed (1.3 ng l⁻¹) than that found by the classical continuous mode (0.3 ng l⁻¹). The aforementioned methodologies were applied to the determination of Hg in water samples having obtained comparable values by both procedures and with those found by an external laboratory.     

Improvements in the methylmercury extraction from human hair by headspace solid-phase microextraction followed by gas-chromatography cold-vapour atomic fluorescence spectrometry

Improvements in the methylmercury extraction from human hair by solid-phase microextraction followed by gas chromatography coupled to cold-vapour atomic fluorescence spectrometry (GC-CVAFS) have been carried out. They consisted in the optimisation of the digestion step prior to the aqueous-phase ethylation and in the GC-CVAFS interface set-up. The main digestion parameters such as acid type, concentration, temperature and time have been optimised for hair sample analysis, thereby avoiding methylmercury degradation. Moreover, the stability of the digested samples was evaluated to improve the sample throughput.     

Comparative study of microwave-induced plasma atomic emission spectrometry and atomic fluorescence spectrometry as gas-chromatographic detectors for the determination of methylmercury in biological samples

In order to attain a lower detection limit with the HS GC MIP analytical method (Head-Space Gas Chromatography with Microwave-Induced Plasma detection) recently developed for the analysis of methylmercury in biological samples, the quarter-wave Evenson-type cavity used until now was replaced by a TM₀₁₀ Beenakker-type cavity, which was used with both argon and helium as carrier gas. With an argon plasma, an eightfold increase in detection limit was gained compared with the argon plasma sustained by the Evenson cavity, while only a four-fold increase was gained with the helium plasma. In a second step of the study, the MIP detector was replaced by an AFS (atomic fluorescence) detector (CVAFS Model-2, Brooks Rand Ltd, Seattle, USA). With this AFS detector a detection limit of 1 ng methyl mercury per g biological tissue could be reached; i.e. measurements were 40 times more sensitive than those using the Evenson cavity. This detector has some other advantages compared with MIP detection: it is less expensive and easier to manipulate, while the same precision and accuracy are obtained. The use of AFS as detector in the headspace gas chromatographic system is therefore an important improvement for the analysis of methyl-mercury in biological samples.     

Improvement of analytical performances for mercury speciation by on-line derivatization, cryofocussing and atomic fluorescence spectrometry

A modified automated on-line hyphenated system for simultaneous inorganic ionic mercury (Hg²⁺) and monomethylmercury (MeHg⁺) analysis by hydride generation (HG) or ethylation (Eth), cryofocussing, gas chromatography (GC) separation and atomic fluorescence spectrometry (AFS) detection has been improved. Both derivatization methods are investigated with respect to the chromatographic and analytical performances. They can be both affected by interferences when the AFS detection system is used. Water vapor removal using a soda lime moisture trap improves significantly the chromatographic performances, the reproducibility and the detection limits for Hg²⁺ and MeHg⁺ analyzed with both methods. For ethylation (Eth) derivatization, a scattering interference generated from low-quality ethylation reagent has also been eliminated. For HG, improved detection limits are 0.13 ng l⁻¹ and 0.01 ng l⁻¹ for Hg²⁺ and MeHg⁺, respectively (0.1 l water sample), and reproducibility are 5% for Hg²⁺ (20 ng l⁻¹) and MeHg⁺ (5 ng l⁻¹). Improved detection limits for Eth are 0.22 ng g⁻¹ for Hg²⁺ and 0.02 ng g⁻¹ for MeHg⁺ (1 g dry sediment sample) and the reproducibility are 5-6% for Hg²⁺ and MeHg⁺ (1-2 ng g⁻¹).     

Voltammetric studies on the electrochemical determination of methylmercury in chloride medium at carbon microelectrodes

Electroanalytical techniques have been used to determine methylmercury at low levels in environmental matrices. The electrochemical behaviour of methylmercury at carbon microelectrodes in a hydrochloric acid medium using cyclic, square wave and fast-scan linear-sweep voltammetric techniques has been investigated. The analytical utility of the methylmercury reoxidation peak has been explored, but the recorded peak currents were found to be poorly reproducible. This is ascribed to two factors: the adsorption of insoluble chloromercury compounds on the electrode surface, which appears to be an important contribution to hinder the voltammetric signal of methylmercury; and the competition between the reoxidation of the methylmercury radical and its dimerization reaction, which limits the reproducibility of the methylmercury peak. These problems were successfully overcome by adopting the appropriate experimental conditions. Fast-scan rates were employed and an efficient electrochemical regeneration procedure of the electrode surface was achieved, under potentiostatic conditions in a mercury-free solution containing potassium thiocyanate—a strong complexing agent. The influence of chloride ion concentration was analysed. Interference by metals, such as lead and cadmium, was considered. Calibration plots were obtained in the micromolar and submicromolar concentration ranges, allowing the electrochemical determination of methylmercury in trace amounts. An estuarine water sample was analysed using the new method with a glassy carbon microelectrode.     

Concentration levels of total and methylmercury in mussel samples collected along the coasts of Sardinia Island (Italy)

This paper reports the assessment of the total mercury (T-Hg) and methylmercury (MeHg) contamination of mussel samples collected by two sampling campaigns from along the coastline of Sardinia (Italy). T-Hg has been determined by a direct mercury analyser (DMA) whereas MeHg has been determined by gas chromatography-mass spectrometry (GC-MS) after acid extraction, and employs a novel NaBPh₄ derivatization method. The evaluation of the quality of measurements was carried out by analysing candidate certified reference material (CRM) BCR 710, for MeHg and T-Hg, and CRM IAEA-350 for T-Hg. In the analysed samples, the T-Hg concentrations range from 35 to 115 μg kg⁻¹ and from 40 to 830 μg kg⁻¹, for the two sampling campaigns, respectively, whereas the MeHg concentrations range from l5 to 51 μg kg⁻¹ and from 17 to 116 μg kg⁻¹. Consequently, the MeHg/T-Hg ratios range from 0.33 to 0.91 and from 0.14 to 0.98, respectively. Despite the increasing trend of Hg concentration from the first to the second sampling campaign, the T-Hg concentration of all the samples was much below the 0.5 μg g⁻¹ WHO limit, and the MeHg values ranged between 2.2 and 17.2 μg kg⁻¹, not exceeding the 43.5 μg kg⁻¹ tolerable daily residue level calculated for Italy.     

Ultratrace determination of mercury in water following EN and EPA standards using atomic fluorescence spectrometry

Chemical vapour generation has been used in combination with atomic fluorescence spectrometry to determine mercury at ultratrace concentrations down to 0.1 ng L^–1. A time-based injection of 1 mL of solution for measurement was sufficient to generate a steady-state detector response in the direct mode of measurement. The detection limit calculated from a ten-point calibration curve according to DIN 32645 was 0.26 ng L^–1. Instrument noise is limited by reflected radiation from the light source rather than by the dark current of the photomultiplier. The detection limit is directly influenced by the reagent blank which was 2 ng L^–1 in the experiments described. Focusing by amalgamation and subsequent thermal desorption generates a detector response which is about eight times higher in peak intensity and about twice as large in integrated intensity. The detection limit under these conditions is 0.09 ng L^–1 which can be further improved by preconcentration of larger volumes of solution for measurement. The cycle time for one individual reading is about 40 s without amalgamation and 125 s with amalgamation. The linear dynamic range of the system is five orders of magnitude with a single photomultiplier gain setting. The carry-over is less than 0.3% in direct measurement mode. Reference water samples and a surface water containing approximately 5 ng L^–1 were used to prove the validity of the method for real samples. Good accuracy and recoveries of 103% were calculated using the fast direct determination technique.     

Comparison of AFS and ICP-MS detection coupled with gas chromatography for the determination of methylmercury in marine samples

Inductively coupled plasma mass spectrometry (ICP-MS) and atomic fluorescence spectrometry (AFS) coupled with gas chromatography (GC) have been evaluated as element specific detectors for the determination of methylmercury in marine samples. Detection limits for methylmercury chloride, obtained using ICP-MS and AFS, were 0.9 and 0.25 pg as Hg, respectively. Methylmercury was determined in marine tissue reference materials IAEA 142 and NIST 8044 mussel homogenate, and DOLT-2 dogfish liver by GC–AFS, with found values of 45±7, 26±4, and 671±41 ng g⁻¹, compared with certified values of 47±4, 28±2, and 693±53 ng g⁻¹. The analyses of IAEA 142 and NIST 8044 were repeated using GC–ICP-MS, with found values of 48±9 and 30±3 ng g⁻¹, respectively. Methylmercury was determined in real samples of ringed seal and beluga whale, with found values of 801±62 and 2830±113 ng g⁻¹, respectively.     

Determination of methylmercury in marine sediment samples: Method validation and occurrence data

The determination of methylmercury (MeHg) in sediment samples is a difficult task due to the extremely low MeHg/THg (total mercury) ratio and species interconversion. Here, we present the method validation of a cost-effective fit-for-purpose analytical procedure for the measurement of MeHg in sediments, which is based on aqueous phase ethylation, followed by purge and trap and hyphenated gas chromatography–pyrolysis–atomic fluorescence spectrometry (GC–Py–AFS) separation and detection. Four different extraction techniques, namely acid and alkaline leaching followed by solvent extraction and evaporation, microwave-assisted extraction with 2-mercaptoethanol, and acid leaching, solvent extraction and back extraction into sodium thiosulfate, were examined regarding their potential to selectively extract MeHg from estuarine sediment IAEA-405 certified reference material (CRM). The procedure based on acid leaching with HNO₃/CuSO₄, solvent extraction and back extraction into Na₂S₂O₃ yielded the highest extraction recovery, i.e., 94 ± 3% and offered the possibility to perform the extraction of a large number of samples in a short time, by eliminating the evaporation step. The artifact formation of MeHg was evaluated by high performance liquid chromatography coupled to inductively coupled plasma mass spectrometry (HPLC–ICP–MS), using isotopically enriched Me²⁰¹Hg and ²⁰²Hg and it was found to be nonexistent. A full validation approach in line with ISO 17025 and Eurachem guidelines was followed. With this in mind, blanks, selectivity, working range (1–800 pg), linearity (0.9995), recovery (94–96%), repeatability (3%), intermediate precision (4%), limit of detection (0.45 pg) and limit of quantification (0.85 pg) were systematically assessed with CRM IAEA-405. The uncertainty budget was calculated and the major contribution to the combined uncertainty (16.24%, k = 2) was found to arise from the uncertainty associated with recovery (74.1%). Demonstration of traceability of measurement results is also presented. The validated measurement procedure was applied to the determination of MeHg incurred in sediments from a highly polluted and scarcely studied area in the Caribbean region.     

Robust microwave-assisted extraction protocol for determination of total mercury and methylmercury in fish tissues

A rapid and efficient closed vessel microwave-assisted extraction (MAE) method based on acidic leaching was developed and optimized for the extraction of total mercury (Hg), inorganic mercury (Hg²⁺) and methylmercury (CH₃Hg⁺) from fish tissues. The quantitative extraction of total Hg and mercury species from biological samples was achieved by using 5 mol L⁻¹ HCl and 0.25 mol L⁻¹ NaCl during 10 min at 60 °C. Total Hg content was determined using inductively coupled plasma mass spectrometry (ICP-MS). Mercury species were measured by liquid chromatography hyphenated with inductively coupled plasma mass spectrometry (LC-ICP-MS). The method was validated using biological certified reference materials ERM-CE464, DOLT-3, and NIST SRM-1946. The analytical results were in good agreement with the certified reference values of total Hg and CH₃Hg⁺ at a 95% confidence level. Further, accuracy validation using speciated isotope-dilution mass spectrometry (SIDMS, as described in the EPA Method 6800) was carried out. SIDMS was also applied to study and correct for unwanted species transformation reactions during and/or after sample preparation steps. For the studied reference materials, no statistically significant transformation between mercury species was observed during the extraction and determination procedures. The proposed method was successfully applied to fish tissues with good agreement between SIDMS results and external calibration (EC) results. Interspecies transformations in fish tissues were slightly higher than certified reference materials due to differences in matrix composition. Depending on the type of fish tissue, up to 10.24% of Hg²⁺ was methylated and up to 1.75% of CH₃Hg⁺ was demethylated to Hg²⁺.     

Simultaneous determination of arsenic and selenium in biological samples by HG-AFS

A new method is proposed for simultaneous determination of traces of arsenic (As) and selenium (Se) in biological samples by hydride-generation double-channel non-dispersive atomic-fluorescence spectrometry (HG-AFS) from tartaric acid media. The effects of analytical conditions on fluorescence signal intensity were investigated and optimized. Interferences from coexisting ions were evaluated. Under optimum conditions linear response ranges above 20 g L^–1 for As and 32 g L^–1 for Se were obtained with detection limits of 0.13 and 0.12 g L^–1, respectively. The precision for elevenfold determination of As at the 4 g L^–1 level and of Se at the 8 g L^–1 level were 2.7 and 1.9% (RSD), respectively. Recoveries of 92.5–95.5% for As and 101.2–108.4% for Se were obtained for four biological samples and two certified biological reference materials. The proposed method has the advantages of simple operation, high sensitivity, and high efficiency; it was successfully used for simultaneous determination of As and Se in biological samples.     

Determination of methylmercury in environmental samples using static headspace gas chromatography and atomic fluorescence detection after aqueous phase ethylation

A rapid and automated method for the determination of monomethylmercury (MMHg) in environmental samples was developed using headspace gas chromatography with atomic fluorescence detection in combination with aqueous phase ethylation. Sample preparation steps were optimized for sediments, biological samples, and water samples using certified reference materials and real samples with a broad range of MMHg concentrations. Different extraction procedures were compared for both sediments and biological samples. The methods were applied in the intercomparison exercises for the certification of MMHg in sediments (IAEA 405) and in Oyster tissue (BCR 710) and the results were accepted for certification. The detection limits for MMHg are 0.002 ng Hg/g for sediments and biological samples and 0.01 ng Hg/L for water samples. The method was tested for methylation artifacts; no artifact was observed in the sediment samples and CRMs tested.     

Optimization of supercritical fluid extraction-gas chromatography of methylmercury in marine samples

Two-level factor designs were used to optimize the supercritical fluid extraction (SFE) of methylmercury (Me---Hg) in marine samples, which were subsequently analysed by gas chromatography-electron capture detection (GC-ECD). Several variables potentially affect to extraction efficiency and kinetics. The factors studied were: CO₂ flow-rate and density, extraction cell temperature, static extraction time, nozzle and trap temperature, amount of hydrochloric acid and contact time between the acid and the sample before to extraction. The extraction kinetics was studied in all experiments by splitting extracts at 2, 7, 17 and 37 min. The results suggest that only the extraction cell temperature is statistically significant. The optimized SFE procedure to extract Me---Hg was validated by means of three available reference materials having certified methylmercury content.     

Application of sequential injection-monosegmented flow analysis (SI-MSFA) to spectrophotometric determination of sulfide in simulated waters samples

This paper describes the coupling of sequential injection with monosegmented flow analysis (SI-MSFA) for determination of sulfide at typical concentrations in wastewaters. The method was based on the reaction of sulfide with 19 mmol l⁻¹ Fe³⁺ and 3.63 mmol l⁻¹N,N-dimethyl-p-phenylene diamine hydrochloride in medium of 1.1 mol l⁻¹ HCl, forming the dye methylene blue. The analytical curves were constructed by in-line dilution of a single stock standard solution. The robustness of the proposed method was checked constructing analytical curves in different working days and comparing the slopes, which had a relative standard deviation of 5.2% (n=5) for a concentration range between 0.17 and 1.0 mg l⁻¹ S²⁻. The analytical throughput was 38 samples per h and the limit of detection was 0.040 mg l⁻¹. The feasibility of the SI-MSFA approach to perform standard additions for S²⁻ determination was also described. Simulated samples spiked with known amounts of sulfide were analyzed by the proposed method, presenting recoveries between 70 and 115%. These results demonstrate the feasibility of the SI-MSFA method to perform in situ analysis of S²⁻ in automatic monitoring stations.     

Contribution to vapor generation-inductively coupled plasma spectrometric techniques for determination of sulfide in water samples

Vapor generation-inductively coupled plasma-optical emission spectrometry was used for the determination of sulfide in water samples preserved by the addition of a zinc acetate and sodium hydroxide solution. Hydrogen sulfide and acid-volatile sulfides were transformed, by acidification, to a gaseous phase in a vapor generator and subsequently detected by inductively coupled plasma optical emission spectrometry. Compounds interfering with iodometric titration and spectrophotometric determination were examined as potential chemical interferents. The proposed method provides results comparable to iodometric titration in the tested concentration range 0.06-22.0 mg L⁻¹. Limit of detection for the determination of hydrogen sulfide by this method is 0.03 mg L⁻¹.     

Determination of mercury in environmental and biological samples by cold vapour atomic absorption spectrometry

A continuously operating monitoring method for total mercury at sub-ng/ml level in environmental and biological samples by cold vapour atomic-absorption spectrometry with NaBH₄ as a reductant was developed. The mercury vapour generator and absorption cell closed-end by quartz were used in this study. The detection limit (S/N = 3) and relative standard deviation of 12 determinations of 10 ng/ml Hg(II) were 0.11 ng/ml and 1.1%, respectively. The range of standard calibration curve was 0–50 ng/ml Hg, The proposed method was successfully applied to the completely continuous monitoring of total mercury in waste water, sediments and pork liver.     

Development of a reference measurement procedure for the determination of methylmercury in fish products

The development of an analytical procedure for speciation analysis of methylmercury in fish products is presented. The method is based on high-performance liquid chromatography hyphenated to inductively coupled plasma-mass spectrometry. The metrological approach is stressed out in this paper, in order to provide reliable and comparable results. A complete uncertainty budget has been evaluated and the method has been validated by the use of a certified reference material. Moreover, the detection could rely on the isotope dilution mass spectrometry, a powerful strategy capable of highly accurate results traceable to the “Système International d’Unités” and recognised by the “Comité Consultatif pour la Quantité de Matière” as a primary method of measurement. Presented at MEFNM 2008, September 2008, Budapest, Hungary.     

Inorganic mercury and methylmercury determination in polluted waters by HPLC coupled to cold vapour atomic fluorescence spectroscopy

A systematic study of Hg²⁺ and CH₃Hg⁺ (MeHg⁺) speciation using hyphenated techniques, was performed for high-performance liquid chromatography coupled to on-line UV irradiation and cold-vapour atomic fluorescence spectroscopy (HPLC-UV-CV-AFS). First, a comparative study of the behaviour of three mobile phase compositions (using tetrabutylammonium bromide (TBAB), L-cysteine and ammonium pyrrolidinedithiocarbamate (APDC)) is presented. The separation and detection system was optimised by considering factors that modify fluorescence signal and the separation such as, the addition of different percentages of an organic modifier (methanol (MeOH) and acetonitrile (ACN)) to the mobile phase, the type of reducing agent used (SnCl₂ and NaBH₄) and the potential memory effects of the material of which the injection system is made (stainless steel, PEEK). The mobile phase selected for its sensitivity was a mixture 80?:?20 MeOH?:?0.0015?mol?l^–1 APDC and 0.01?mol?l^–1 NH₄CH₃COO (pH 5.5). The detection and quantification limits were close to 1.5 and 5?µg?l^?1 for both species (as Hg), respectively. Recoveries obtained using fortified water samples of distinct origin (soft mineral, tap, river, seawater, and wastewater), ranged from 90 to 115% for concentrations about 2 and 20 times over quantification limits. Good repeatability was obtained (about 5%) independently of the concentrations, with reproducibility values about 20% at low concentrations and 5–10% at higher concentrations. Our proposed method proved to be straightforward for use by environmental laboratories for routine Hg²⁺ and MeHg⁺ determinations in polluted water samples.