Effect of the interface on separation in multicapillary gas chromatography-based hyphenated techniques for speciation analysis of organometallic compounds

This paper reports the effect of transfer line (TL) internal diameter (i.d.) on gas chromatographic separation characteristics such as efficiency and speed, when a multicapillary (MC) column is used for speciation analysis of mercury. Five different TL consisting of fused-silica capillaries with 0.15, 0.20, 0.25, 0.32, and 0.53 mm i.d. are compared. The separation efficiency and total chromatographic run time are critically affected by the i.d. of the TL. Narrow capillaries (i.d.0.20 mm) produce minimum peak dispersion whereas wide capillaries result in narrow peaks and shorter chromatographic analysis times. A thermodynamic approach is proposed to describe the motion of the analytes through the separation column and TL. The model provides good agreement with the experimental data for high pressures (35 psig) and wide TL (0.25 mm i.d.).Dedicated to the memory of Wilhelm Fresenius     

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.     

Comparative study of atomic fluorescence spectroscopy and inductively coupled plasma mass spectrometry for mercury and arsenic multispeciation

Mercury and arsenic are two elements of undoubted importance owing to their toxic character. Although speciation of these elements has been developed separately, in this work for the first time the speciation of As and Hg using two atomic fluorescence detectors in a sequential ensemble is presented. A coupling based on the combination of high-performance liquid chromatography (where mercury and arsenic species are separated) and two atomic fluorescence detectors in series, with several online treatments, including photooxidation (UV) and hydride generation, has allowed the determination of mercury and arsenic compounds simultaneously. The detection limits for this device were 16, 3, 17, 12 and 8 ng mL^–1 for As^III, monomethylarsinic acid, As^V, Hg²⁺ and methylmercury, respectively. This coupling was compared with an analogous one based on inductively coupled plasma–mass spectrometry (ICP-MS) detection, with detection limits of 0.7, 0.5, 0.8, 0.9 and 1.1 ng mL^–1, respectively. Multispeciation based on ICP-MS exhibits better sensitivity than the coupling based on tandem atomic fluorescence, but this second device is a very robust system and exhibits obvious advantages related to the low cost of acquisition and maintenance, as well as easy handling, which makes it a suitable system for routine laboratories.     

Multicapillary gas chromatography coupled to inductively coupled plasma-time-of-flight mass spectrometry for rapid mercury speciation analysis

A simple, rapid and accurate method on the basis of multicapillary gas chromatography (MCGC) combined with inductively coupled plasma-time-of-flight mass spectrometry (ICP-TOFMS) was developed for speciation analysis of methylmercury (MeHg⁺) and inorganic mercury (Hg²⁺). The potential of the ICP-TOFMS for transient multi-isotope detection of very short signals (peak width of 0.4 s at half peak height) was evaluated. Two injection systems (purge-and-trap (PTI) and split (SI) injections) were compared in terms of species separation resolution and transient signal profile. Using purge-and-trap injection, after in situ derivatization of the ionic mercury species with sodium tetraethylborate, a baseline separation of MeHg⁺ and Hg²⁺ was achieved within a chromatographic run of <35 s. To correct for matrix-induced ion signal variation and instrumental drift, propylmercury (PrHg⁺) was used as internal standard. Detection limits of 16 and 257 fg g⁻¹ for MeHg⁺ (as Hg) and Hg²⁺, respectively, were achieved. The analytical precision (R.S.D. (%)) for 10 successive injections of a standard mixture containing 10 pg MeHg⁺ (as Hg) and Hg²⁺ was 1.2% for MeHg⁺ and 4.1% for Hg²⁺. The method was validated by analysis of two biological certified reference materials (CRM): a dogfish muscle (DORM-2) and a freeze-dried tuna fish (CRM 464).     

Determination of mercurial species in fish by inductively coupled plasma mass spectrometry with anion exchange chromatographic separation

This work demonstrated the feasibility of mercury speciation analysis by anion exchange chromatographic separation with inductively coupled plasma mass spectrometry detection. For the first time, by complexing with the mobile phase containing 3-mercapto-1-propanesulfonate into negatively charged complexes, fast separation of inorganic mercury (Hg²⁺), monomethylmercury (MeHg), ethylmercury (EtHg) and phenylmercury (PhHg) was achieved within 5 min on a 12.5-mm strong anion exchange column. The detection limits for Hg²⁺, MeHg, EtHg and PhHg were 0.008, 0.024, 0.029 and 0.034 μg L⁻¹, respectively. The relative standard deviations of peak height and peak area (5.0 μg L⁻¹ for each Hg species) were all below 3%. The determined contents of Hg²⁺, MeHg and total Hg in a certified reference material of fish tissue by the proposed method were in good accordance with the certified values with satisfactory recoveries. The relative errors for determining MeHg and total mercury were −2.4% and −1.2%, respectively, with an acceptable range for spike recoveries of 94–101%. Mercury speciation in 11 fish samples were then analyzed after the pretreated procedure. The mercury contents in all fish samples analyzed were found compliant with the criteria of the National Standards of China.     

Development of a new hybrid technique for rapid speciation analysis by directly interfacing a microfluidic chip-based capillary electrophoresis system to atomic fluorescence spectrometry

This paper represents the first study on direct interfacing of microfluidic chip-based capillary electrophoresis (chip-CE) to a sensitive and selective detector, atomic fluorescence spectrometry (AFS) for rapid speciation analysis. A volatile species generation technique was employed to convert the analytes from the chip-CE effluent into their respective volatile species. To facilitate the chip-CE effluent delivery and to provide the necessary medium for subsequent volatile species generation, diluted HCl solution was introduced on the chip as the makeup solution. The chip-CE-AFS interface was constructed on the basis of a concentric "tube-in-tube" design for introducing a KBH4 solution around the chip effluent as sheath flow and reductant for volatile species generation as well. The generated volatile species resulting from the reaction of the chip-CE effluent and the sheath flow were separated from the reaction mixture in a gas-liquid separator and swept into the AFS atomizer by an argon flow for AFS determination. Inorganic mercury (Hg(II)) and methylmercury (MeHg(I)) were chosen as the targets to demonstrate the performance of the present technique. Both mercury species were separated as their cysteine complexes within 64 s. The precision (relative standard deviation, RSD, n = 5) of migration time, peak area, and peak height for 2 mg.L(-1) Hg(II) and 4 mg.L(-1) MeHg(I) (as Hg) ranged from 0.7 to 0.9%, 2.1 to 2.9%, and 1.5 to 1.8%, respectively. The detection limit was 53 and 161 microg.L(-1) (as Hg) for Hg(II) and MeHg(I), respectively. The recoveries of the spikes of mercury species in four locally collected water samples ranged from 92 to 108%.     

Method optimization for the determination of four mercury species by micro-liquid chromatography-inductively coupled plasma mass spectrometry coupling in environmental water samples

A method based on the coupling microHPLC-microneb-ICPMS has been developed for Hg(II), MeHg⁺, EtHg⁺ and PhHg⁺ species. Gradient elution using methanol and l-cysteine at pH 3.0 allowed the chromatographic separation of all species in less than 13 min (total analysis time 15 min). The direct coupling of microLC to ICPMS through a Micromist nebulizer permits the analysis of environmental water without sample pretreatment and derivatization steps. Nebulizer type, organic modifier and column length were the main parameters tested. The methanol content and pH of the mobile phase greatly affected the retention time and sensitivity of the method. Key factors to obtain high signal to noise ratio, at concentrations below 1 μg L⁻¹, were found to be the nebulization step and traces of Hg present in the complexing agent. A detailed optimization of carrier and make up gas flow rates have enabled the nebulization of the methanol gradient elution with good mass transport efficiency, low organic solvent loading into the plasma and excellent precision.The performance of the microHPLC-microneb-ICPMS method developed was evaluated on a surface water sample filtered (0.22 μm) and spiked with 0.5 μg L⁻¹ (as Hg) of each species. Precision (R.S.D., n = 6) for all species of Hg varied from 0.5 to 2.1%. Detection limit, defined as three times the standard deviation (n = 6), ranged from 8 ng L⁻¹ for EtHg⁺ to 32 ng L⁻¹ for PhHg⁺ and was noticeably lower than those reported in previous LC-based methods. Accuracy was suitable with recoveries ranging from 85 to 100% when tested at two levels (0.5 and 10 μg L⁻¹) in groundwater samples. Recovery was matrix affected when water samples of high salinity (depurated wastewater and seawater) were used.     

Trends in selenium determination/speciation by hyphenated techniques based on AAS or AFS

The field of selenium speciation has been studied for decades and the growing interest in this field seems never to reach a plateau. Although powerful techniques based on mass spectrometry are nowadays used for selenium determination/speciation, few laboratories can support the high cost of such techniques. The hyphenation of chromatography to atomic absorption or atomic fluorescence spectrometry (AAS or AFS) is still a reliable and low-cost alternative for routine laboratories. In this work we present the most important parameters dealing with selenium speciation along with the latest trends in this subject, namely in the items related with sample treatment and hyphenation techniques with AAS and AFS detection.     

Mercury speciation in thawed out and refrozen fish samples by gas chromatography coupled to inductively coupled plasma mass spectrometry and atomic fluorescence spectroscopy

Different sub-sampling procedures were applied for the determination of mercury species (as total mercury Hg, methylmercury MeHg⁺ and inorganic mercury Hg²⁺) in frozen fish meat. Analyses were carried out by two different techniques. After the sample material was pre-treated by microwave digestion, atomic fluorescence spectroscopy (AFS) was used for the determination of total Hg. Speciation analysis was performed according to the following procedure: dissolution of sample material in tetramethylammonium hydroxide (TMAH), derivatisation with sodium tetraethylborate (NaBEt₄), extraction into isooctane and measurement with gas chromatography inductively coupled plasma mass spectrometry (GC-ICPMS) for the identification and quantification of methylmercury (MeHg⁺) and inorganic mercury (Hg²⁺). The concentration range of total Hg measured in the shark fillets is between 0.9 and 3.6 g g^–1 thawed out shark fillet. Speciation analysis leads to 94% Hg present as MeHg⁺. Homogeneity, storage conditions and stability of analytical species and sample materials have great influence on analytical results. Sub-sampling of half-frozen/partly thawed out fish and analysis lead to significantly different concentrations, which are on average a factor of two lower.     

Capillary electrophoresis on-line coupled with hydride generation-atomic fluorescence spectrometry for speciation analysis of selenium

A new method for speciation analysis of two inorganic selenium species was developed by on-line coupling of capillary electrophoresis (CE) with hydride generation-atomic fluorescence spectrometry (HG-AFS) and on-line conversion of Se(VI) to Se(IV). Baseline separation of Se(VI) and Se(IV) was achieved by CE in a 50 cm x 75 microm inside diameter (ID) fused-silica capillary at -20 kV using a mixture of 15 mmol.L(-1) NaH2PO4 and 0.5 mmol.L(-1) cetyltrimethylammonium bromide (pH 7.5) as electrolyte buffer. Se(VI) was on-line reduced to Se(IV) by mixing the CE effluent with concentrated HCl. The precision (relative standard deviation, RSD, n=7) ranged from 0.7 to 1.3% for migration time, 6.4 to 3.7% for peak height response, and 5.9 to 6.1% for peak area for the two selenium species at the 500 microg.L(-1) (as Se) level. The detection limits were 33 and 25 microg.L(-1) (as Se) for Se(VI) and Se(IV), respectively. The recoveries of the two selenium species in five locally collected water samples ranged from 88 to 114%. The developed method was applied to speciation analysis of inorganic selenium species in spiked natural water samples.     

环境领域铊元素的分析技术研究进展EI北大核心CSCD

铊是一种剧毒的蓄积性重金属元素。伴随着含铊矿物资源的开发利用,铊向环境中的迁移已不容忽视,环境铊污染事件时有发生。铊的分析技术对铊污染的防治具有重要意义。环境领域铊的分析技术近年来也有了新的发展。重点对环境水体、土壤、大气中铊元素分析技术的近期发展进行了综述。在电感耦合等离子体-质谱(ICP-MS)、石墨炉原子吸收光谱(GF-AAS)法为主流分析手段的同时,随着铊新型富集技术的应用以及仪器性能的提升,环境铊分析技术呈现出高灵敏、高稳定性的趋势。针对环境领域铊元素分析技术的发展,提出环境样品铊的化学及赋存形态分析、铊的在线监测、与铊高效富集技术的联用以及环境固体废物中铊的分析是其重要的发展方向。     

Reporting of variations in the natural isotopic composition of mercury

High-precision measurements of natural variations in the stable isotopic composition of mercury show great promise as a new tracer of mercury sources and chemical transformations in the environment. We strongly suggest that all laboratories adopt a common means of data correction, standardization, and nomenclature in order to ensure that data from various laboratories can be easily evaluated and compared. We make suggestions for mass bias correction, reporting of mass-dependent and mass-independent isotope variations, and a standard protocol for reporting analytical uncertainties. We also present our measured values for isotope ratios in several mercury standard solutions.     

气相色谱-电感耦合等离子体质谱

从接口设计、色谱和质谱技术的应用和实际应用等方面对气相色谱－电感耦合等离子体质谱的进展进行了介绍。     

Extraction tool and matrix effects on arsenic speciation analysis in cell lines

Arsenic glutathione (As–GSH) complexes have been suggested as possible metabolites in arsenic (As) metabolism. Extensive research has been performed on the toxicological and apoptotic effects of As, while few reports exist on its metabolism at the cellular level due to the analytical challenges. In this study, an efficient extraction method for arsenicals from cell lines was developed. Evaluation of extraction tools; vortex, ultrasonic bath and ultrasonic probe and solvents; water, chemicals (methanol and trifluoroacetic acid), and enzymes (pepsin, trypsin and protease) was performed. GSH effect on the stability of As–GSH complexes was studied. Arsenic metabolites in dimethylarsino glutathione (DMA(GS)) incubated multiple myeloma cell lines were identified following extraction. Intracellular GSH concentrations of myeloma cell lines were imitated in the extraction media and its corresponding effect on the stability and distribution of As metabolites was studied. An enhancement in both extraction recoveries and time efficiency with the use of the ultrasonic probe was observed. Higher stabilities for the As species in water, pepsin and trypsin were obtained. The presence of 0.5 mM GSH in the extraction media (PBS, pH 7.4) could not stabilize the As–GSH complexes compared to the 5 mM GSH, where high stabilization of the complexes was observed over a 5 day storage study. Finally, the speciation analysis of the DMA(GS) culture incubated cell lines in the presence or absence of GSH revealed the important role GSH plays in the preservation of DMA(GS) identity. Hence, caution is required during the extraction of arsenicals especially the As–GSH complexes, since their identification is highly dependent on GSH concentration.     

Complementary chromatography separation combined with hydride generation-inductively coupled plasma mass spectrometry for arsenic speciation in human urine

This study aimed to establish complementary high performance liquid chromatography (HPLC) methods including three modes of separation: ion pairing, cation exchange, and anion exchange chromatography, with detection by inductively coupled plasma mass spectrometry (ICPMS). The ion pairing mode enabled the separation of inorganic arsenate (As(V)), monomethylarsonic acid (MMA(V)), and dimethylarsinic acid (DMA(V)). However, the ion pair mode was unable to differentiate inorganic arsenite (As(III)) from arsenobetaine (AsB); instead, cation exchange chromatography was used to isolate and quantify AsB. Anion exchange chromatography was able to speciate all of the aforementioned arsenic species. Potential inaccurate quantification problem with urine sample containing elevated concentration of AsB, which eluted immediately after As(III) in anion exchange or ion pairing mode, was overcame by introducing a post-column hydride generation (HG) derivatization step. Incorporating HG between HPLC and ICPMS improved sensitivity and specificity by differentiating AsB from hydride-forming arsenic species. This paper emphasizes the usefulness of complementary chromatographic separations in combination with HG-ICPMS to quantitatively determine concentrations of As(III), DMA(V), MMA(V), As(V), and AsB in the sub-microgram per liter range in human urine.     

Analysis and leaching characteristics of mercury and arsenic in Chinese medicinal material

The purpose of this study is to investigate the amounts and characteristics of heavy metals (As, Hg) leachable from several Chinese medicinal materials (CMM) under conditions simulating stomach and intestine digestion and absorption. Analysis by inductively coupled plasma mass spectrometry (ICP-MS) was compared with that by hydride generation atomic fluorescence spectrometry (HG-AFS). Focused microwave assisted extraction (MAE) and Soxhlet extraction were carried out to compare with the conventional sequential extraction method. The CMM studied included two mineral drugs: realgar and cinnabar, and two formulated drugs containing the two minerals. The leachable amounts of the target elements into artificial stomach fluid, artificial intestinal fluid, and artificial intestinal fluid in 0.5% trypsin were compared. The last solvent gave the greatest amounts of leachable As (0.41%) from realgar and Hg (1×10⁻⁴%) from cinnabar, but otherwise no significant effect on the leachable amounts was observed upon changing the following parameters: temperature (37-60 °C), HCl concentration (0.5-6 M), and CMM sample particle size (74 and 250 μm). The low leaching efficiencies observed confirmed the presence of As and Hg as insoluble species (sulfides)in these mineral drugs. Sequential extraction schemes were used to determine the species of mercury and arsenic in formulated drugs containing the minerals. Trace amounts of organic forms of arsenic (0.43%) and mercury (2.9×10⁻⁴%) were observed which could be the transformation products derived from the original cinnabar or realgar minerals in drug formulation.     

Stability of arsenic peptides in plant extracts: off-line versus on-line parallel elemental and molecular mass spectrometric detection for liquid chromatographic separation

The instability of metal and metalloid complexes during analytical processes has always been an issue of an uncertainty regarding their speciation in plant extracts. Two different speciation protocols were compared regarding the analysis of arsenic phytochelatin (As^IIIPC) complexes in fresh plant material. As the final step for separation/detection both methods used RP-HPLC simultaneously coupled to ICP-MS and ES-MS. However, one method was the often used off-line approach using two-dimensional separation, i.e. a pre-cleaning step using size-exclusion chromatography with subsequent fraction collection and freeze-drying prior to the analysis using RP-HPLC–ICP-MS and/or ES-MS. This approach revealed that less than 2% of the total arsenic was bound to peptides such as phytochelatins in the root extract of an arsenate exposed Thunbergia alata, whereas the direct on-line method showed that 83% of arsenic was bound to peptides, mainly as As^IIIPC₃ and (GS)As^IIIPC₂. Key analytical factors were identified which destabilise the As^IIIPCs. The low pH of the mobile phase (0.1% formic acid) using RP-HPLC–ICP-MS/ES-MS stabilises the arsenic peptide complexes in the plant extract as well as the free peptide concentration, as shown by the kinetic disintegration study of the model compound As^III(GS)₃ at pH 2.2 and 3.8. But only short half-lives of only a few hours were determined for the arsenic glutathione complex. Although As^IIIPC₃ showed a ten times higher half-life (23 h) in a plant extract, the pre-cleaning step with subsequent fractionation in a mobile phase of pH 5.6 contributes to the destabilisation of the arsenic peptides in the off-line method. Furthermore, it was found that during a freeze-drying process more than 90% of an As^IIIPC₃ complex and smaller free peptides such as PC₂ and PC₃ can be lost. Although the two-dimensional off-line method has been used successfully for other metal complexes, it is concluded here that the fractionation and the subsequent freeze-drying were responsible for the loss of arsenic phytochelatin complexes during the analysis. Hence, the on-line HPLC–ICP-MS/ES-MS is the preferred method for such unstable peptide complexes. Since freeze-drying has been found to be undesirable for sample storage other methods for sample handling needed to be investigated. Hence, the storage of the fresh plant at low temperature was tested. We can report for the first time a storage method which successfully conserves the integrity of the labile arsenic phytochelatin complexes: quantitative recovery of As^IIIPC₃ in a formic acid extract of a Thunbergia alata exposed for 24 h to 1 mg As^v L⁻¹ was found when the fresh plant was stored for 21 days at 193 K. Figure On-line HPLC–ICP-MS/ES-MS (bottom) is the preferred method for MS determination of unstable arsenic peptide complexes in plant extracts, since this avoids fractionation and subsequent freeze-drying that are responsible for loss of arsenic phytochelatin complexes in the 2D off-line method (top) Electronic supplementary material  The online version of this article (doi:) contains supplementary material, which is available to authorized users.     

A multinjection strategy for mercury speciation

A multiinjection strategy has been developed to increase the sampling throughput of the high-performance liquid chromatography determination of inorganic-mercury, methylmercury, ethylmercury and phenylmercury. The method involves the injection of samples each 3.5 min, in spite of the fact that phenylmercury retention time corresponds to 9.04 min. In the selected conditions, the sampling frequency was 11 h⁻¹ in front of that of 6 h⁻¹, obtained by conventional injection of each sample after the complete elution of Hg species. Additionally, the analytical reagents consumption was reduced drastically in almost 50%. The main characteristics of the chromatographic separation were maintained and only the resolution of phenylmercury was reduced from 10.3 to 1.7 and that of ethylmercury from 4.6 to 3.1.     

Comparison of gas chromatographic and gas chromatographic/mass spectrometric techniques for the analysis of TNT and related nitroaromatic compounds

The use of capillary column gas chromatography and gas chromatography/mass spectrometry for the analysis of a series of standard solutions (0.1 to 10 μg/ml) of 2,4,6-trinitrotoluene (TNT) and eight other nitroaromatic components was evaluated. The techniques included gas chromatography with electron capture detection (GC/ECD), full scan and selected ion monitoring gas chromatography/mass spectrometry with electron impact ionization (EI/FS and EI/SIM), full scan and selected ion monitoring gas chromatography/mass spectrometry with positive ion chemical ionization using methane reagent gas (PICI/FS and PICI/SIM), and full scan and selected ion monitoring gas chromatography/mass spectrometry with negative ion chemical ionization using methane reagent gas (NICI/FS and NICI/SIM). The performance of the techniques was comapared by determining the linear response range, precision, and detection limits of the analyses.     

Arsenic speciation in Chinese brake fern by ion-pair high-performance liquid chromatography-inductively coupled plasma mass spectroscopy

Ion-pair reverse-phase HPLC-inductively coupled plasma (ICP) MS was employed to determine arsenite [As(III)], dimethyl arsenic acid (DMA), monomethyl arsenic (MMA) and arsenate [As(V)] in Chinese brake fern (Pteris vittata L.). The separation was performed on a reverse-phase C18 column (Haisil 100) by using a mobile phase containing 10 mM hexadecyltrimethyl ammonium bromide (CTAB) as ion-pairing reagent, 20 mM ammonium phosphate buffer and 2% methanol at pH 6.0. The detection limits of arsenic species with HPLC-ICP-MS were 0.5, 0.4, 0.3 and 1.8 ppb of arsenic for As(III), DMA, MMA, and As(V), respectively. MMA has been shown for the first time to experimentally convert to DMA in the Chinese brake fern, indicating that Chinese brake fern can convert MMA to DMA by methylation.