Selenium speciation from food source to metabolites: a critical review

Especially in the last decade, a vast number of papers on Se and its role in health issues have been published. This review gives a brief, critical overview of the main analytical findings reported in these papers. Of particular interest is the Se content in different food sources worldwide and the extent to which their consumption is reflected in the Se content of human tissues and body fluids. Several food sources, both natural (Brazil nuts, garlic, Brassica juncea) and Se-enriched (yeast-based supplements), are discussed as to origin, characteristics, Se metabolism and impact of their consumption on the human body. The continuous development of new and improvement of existing analytical techniques has provided different powerful tools to unravel the Se species and their function. An up-to-date literature study on Se speciation analysis is given, illustrating how analytical chemistry in its different facets aids in the identification of Se compounds and provides insight into the complete metabolic pathway of Se throughout the human body. This review includes a detailed image of the current state-of-the-art of Se speciation analysis in these food sources and in human tissues and body fluids.     

Enzymatic probe sonication as a tool for solid-liquid extraction for total selenium determination by electrothermal-atomic absorption spectrometry

A new fast and reproducible approach is described for the application of the enzymatic probe sonication (EPS) methodology [J.L. Capelo, P. Ximénez-Embún, Y. Madrid-Albarrán, C. Cámara, Anal. Chem. 76 (2004) 233-237] for total selenium determination by electrothermal atomic absorption spectrometry, ET-AAS. Ni(NO₃)₂ and Pd(NO₃)₂ were studied as matrix modifiers in conjunction with H₂O₂, being best results obtained with Pd(NO₃)₂ plus H₂O₂. The presence of H₂O₂ as matrix modifier increases up to 66% the time-life of the graphite tubes, by avoiding the building-up of carbonaceous residues. BCR-414 plankton and ERM-CE 278 mussel tissue reference materials were used for proof-of-the-methodology. Different enzymes, protease XIV, substilisin and trypsin were studied. The use of fresh enzyme was found critical. Good Se recoveries were obtained for oyster tissue, 111%; BCR-414 plankton, 106% and ERM-CE 278 mussel tissue, 93%, when protease XIV was used. Data regarding microwave digestion versus EPS methodology is also presented and discussed.     

Separation and speciation of selenium in food and water samples by the combination of magnesium hydroxide coprecipitation-graphite furnace atomic absorption spectrometric determination

A simple and economic separation and speciation procedure for selenium in food and water samples have been presented prior to its graphite furnace atomic absorption spectrometry (GFAAS). Magnesium hydroxide coprecipitation system for selenium(IV) was applied to the separation and speciation of selenium ions. The influences of the various analytical parameters for the quantitative recoveries of selenium ions like pH, amounts of magnesium ions as carrier elements, etc. on were examined. The effects of the alkaline and earth alkaline metals, some transition metals and some anions on the recoveries of selenium(IV) were also investigated. The recoveries of analytes were found greater than 95%. No appreciable matrix effects were observed. The detection limit, defined as three times the blank standard deviation (3σ), was 0.030 μg l⁻¹. The preconcentration factor for the presented system was 25. The proposed method was applied to the speciation of selenium(IV), selenium(VI) and determination of total selenium in natural waters and microwave digested various food samples with satisfactory results. The procedure was validated with certified reference materials. The relative errors and relative standard deviations were below 6% and 10%, respectively.     

Optimisation of sample treatment for arsenic speciation in alga samples by focussed sonication and ultrafiltration

A procedure for arsenic species fractionation in alga samples (Sargassum fulvellum, Chlorella vulgaris, Hizikia fusiformis and Laminaria digitata) by extraction is described. Several parameters were tested in order to evaluate the extraction efficiency of the process: extraction medium, nature and concentration (tris(hydroxymethyl)aminomethane, phosphoric acid, deionised water and water/methanol mixtures), extraction time and physical treatment (magnetic stirring, ultrasonic bath and ultrasonic focussed probe). The extraction yield of arsenic under the different conditions was evaluated by determining the total arsenic content in the extracts by ICP-AES. Arsenic compounds were extracted in 5 mL of water by focussed sonication for 30 s and subsequent centrifugation at 14,000 × g for 10 min. The process was repeated three times. Extraction studies show that soluble arsenic compounds account for about 65% of total arsenic.

An ultrafiltration process was used as a clean-up method for chromatographic analysis, and also allowed us to determine the extracted arsenic fraction with a molecular weight lower than 10 kDa, which accounts for about 100% for all samples analysed.

Speciation studies were carried out by HPLC–ICP-AES. Arsenic species were separated on a Hamilton PRP-X100 column with 17 mM phosphate buffer at pH 5.5 and 1.0 mL min⁻¹ flow rate. The chromatographic method allowed us to separate the species As(III), As(V), MMA and DMA in less than 13 min, with detection limits of about 20 ng of arsenic per species, for a sample injection volume of 100 μL. The chromatographic analysis allowed us to identify As(V) in Hizikia (46 ± 2 μg g⁻¹), Sargassum (38 ± 2 μg g⁻¹) and Chlorella (9 ± 1 μg g⁻¹) samples. The species DMA was also found in Chlorella alga (13 ± 1 μg g⁻¹). However, in Laminaria alga only an unknown arsenic species was detected, which eluted in the dead volume.     

Cyclic neutron activation analysis for determination of selenium in food samples using <Superscript>77m</Superscript>Se

Cyclic neutron activation analysis method was conducted for determination of Se in food samples. High accuracy and good precision were proved by analyzing certified reference materials (CRMs) of chicken (GBW10018), rice (GBW10010) and cabbage (GBW10014). The detection limits for the three CRMs reached 0.16, 0.66 and 1.2 ng after 6 cycles at the 161.9 keV γ-peak from ^77mSe, under a neutron flux of 9.0 × 10¹¹ n cm⁻² s⁻¹ and the conditions of 30 s irradiation, 2 s decay, 30 s counting and 2 s waiting, significantly lower than those of conventional neutron activation analysis without any cycles, which were 0.94, 3.6 and 4.3 ng, respectively.     

Precipitate flotation-separation, speciation and hydride generation atomic absorption spectrometric determination of selenium(IV) in food stuffs

A method for flotation and determination of selenium(IV) in foodstuffs using p-chlorophenylthiosemicarbazide (HCPT) was investigated. At pH  2, selenium(IV) forms a 1:1 reddish-brown precipitate with HCPT easily floated using oleic acid (HOL) surfactant. The separated complex was dissolved in 4 M HCl and diluted in 10-ml double-distilled water (DDW). Selenium(IV) content in the eluate was determined by hydride generation atomic absorption spectrometry (HG-AAS) at 196.4 nm using sodium borohydride. The HCPT–Se(IV) complexes formed in absence and presence of oleic acid were characterized by elemental analysis, mass and infrared spectral studies. The mode of chelation between Se(IV) and HCPT is proposed to be through S and N coordination. Interferences, on the flotation process, from various foreign ions were avoided by adding excess HCPT. The proposed flotation methodology was successfully applied to the analysis of selenium in real foodstuffs and natural water spiked with known amounts of Se(IV) with a preconcentration factor of 100 and a detection limit of 20 pg. Application was also extended to separate Se(IV) successfully from Se(VI) in their synthetic mixtures. The separation mechanism is proposed to be due to hydrogen bond formation between the COOH group of HOL and –NH of the HCPT–Se(IV) complex.     

Factors affecting arsenic speciation in environmental samples: sample drying and storage

Arsenic is a ubiquitous element. Its toxicity, mobility, and bioaccumulation depend usually on its chemical form, and therefore, arsenic speciation is indispensable for the assessment of environmental risk and human hazard. Little is known about the effect of sample preparation procedures, such as drying and storage, on the resulting arsenic speciation. In this study, we investigated the influence of different drying methods and storage conditions on the arsenic speciation in mineral soils, organic soils, and plants. Drying soils and plants using different methods may change the concentrations of the total methanol–water (20%,?v/v) extractable arsenic, the proportion of organic arsenic and the ratio of arsenite-to-arsenate. Loss of methanol–water extractable arsenic compounds (up to 63%) was observed particularly in the samples rich in water. Following drying, the speciation of organic arsenic changed less than that of inorganic arsenic. Drying showed little influence on the total arsenic determination. None of the storage methods tested could preserve the arsenic speciation in organic soils and plants, although arsenic speciation after one-month storage varied less in freeze-dried samples than wet samples. Storage of the samples at low temperatures (2 or??20°C) had the largest impact on the samples rich in organic matters, leading to less arsenic being extractable by methanol–water. Both drying and storage of the soil and plant samples changed apparently the arsenic speciation. Therefore, we recommend conducting the arsenic speciation possibly with fresh and wet samples, so that the results of arsenic speciation may be more approaching the original states.     

Determination of selenium in food matrices by replicate sample neutron activation analysis

The replicate sample instrumental neutron activation method was optimized and used for the determination of selenium in foodstuffs. The method was reliable, yielding accurate results. Lower detections limits were obtained after each successive irradiation. Different irradiation conditions were used depending on the type of sample. For samples with higher selenium contents (meat, fish, eggs), the measured selenium in the first replicate is in all cases larger than the detection limit, but a better accuracy was obtained with a larger number of replicates (2–3 replicates). For samples with extremely low selenium contents (vegetable samples), at least seven replicates were necessary to obtain a concentration value two times larger than the detection limit.     

Preconcentration of selenium compounds on a porous graphitic carbon column in view of HPLC-ICP-AES speciation analysis

The retention of organic selenium compounds on a porous graphitic carbon stationary phase was investigated. Different acids were studied as mobile phases to elute selenocystamine, selenoethionine, selenomethionine and selenocystine. Detection was achieved using inductively coupled plasma-atomic emission spectrometry to provide selenium-specific and sensitive detection. The separation of the four species was carried out using methanoic acid. An important on-column preconcentration was obtained when solutes were injected in nitric acid or trifluoroacetic acid (TFA) media. The large injection volume employed (2,500 µL) allowed us to reach low relative detection limits (2–6 µg/L). The method, employing TFA as injection solvent and methanoic acid as the eluent was found to be robust with respect to different matrices spiked with selenocompounds.     

Certification of a new selenized yeast reference material (SELM-1) for methionine, selenomethinone and total selenium content and its use in an intercomparison exercise for quantifying these analytes

A new selenized yeast reference material (SELM-1) produced by the Institute for National Measurement Standards, National Research Council of Canada (INMS, NRC) certified for total selenium (2,059±64 mg kg⁻¹), methionine (Met, 5,758±277 mg kg⁻¹) and selenomethionine (SeMet, 3,431±157 mg kg⁻¹) content is described. The ±value represents an expanded uncertainty with a coverage factor of 2. SeMet and Met amount contents were established following a methanesulfonic acid digestion of the yeast using GC-MS and LC-MS quantitation. Isotope dilution (ID) calibration was used for both compounds, using ¹³C-labelled SeMet and Met. Total Se was determined after complete microwave acid digestion based on ID ICP-MS using a ⁸²Se spike or ICP-OES spectrometry using external calibration. An international intercomparison exercise was piloted by NRC to assess the state-of-the-art of measurement of selenomethione in SELM-1. Determination of total Se and methionine was also attempted. Seven laboratories submitted results (2 National Metrology Institutes (NMIs) and 5 university/government laboratories). For SeMet, ten independent mean values were generated. Various acid digestion and enzymatic procedures followed by LC ICP-MS, LC AFS or GC-MS quantitation were used. Four values were based on species-specific ID calibration, one on non-species-specific ID with the remainder using standard addition (SA) or external calibration (EC). For total selenium, laboratories employed various acid digestion procedures followed by ICP-MS, AFS or GC-MS quantitation. Four laboratories employed ID calibration, the remaining used SA or EC. A total of seven independent results were submitted. Results for methionine were reported by only three laboratories, all of which used various acid digestion protocols combined with determination by GC-MS and LC UV. The majority of participants submitted values within the certified range for SeMet and total Se, whereas the intercomparison was judged unsuccessful for Met because only two external laboratories provided values, both of which were outside the certified range.     

Evaluation of different sample extraction strategies for selenium determination in selenium-enriched plants (Alliumsativum and Brassicajuncea) and Se speciation by HPLC-ICP-MS

Several sample extraction techniques have been evaluated in order to obtain highest selenium (Se) extraction efficiency in two types of selenium-enriched plants (Allium sativum and Brassica juncea). Three extracting solutions have been studied for this purpose: 0.1 M HCl, 25 mM ammonium acetate buffer (pH 5.6) and protease in aqueous solution. In each case, the effect of the ultrasonic probe during extraction was also evaluated. Selenium extraction yields were calculated based on the ICP-MS determination of the total selenium content in the corresponding extracts and in the plant tissue after its microwave digestion. The action of ultrasounds allowed the reduction on the extraction time while maintaining good Se recoveries (which ranged from 75 to 120% of the total Se in the plant). The accuracy of total Se determination was controlled by analyzing a reference material (aquatic plant, BCR-670). On the other hand, speciation studies of the extracts were carried out by using ion-pairing reversed phase and size exclusion/ion exchange (Shodex Asshipak) liquid chromatographic columns. The two separation mechanisms were suitable to isolate the main extractable Se species which were identified as Se-methyl selenocysteine and Se-methionine in both systems. The extracts of both plants (A. Sativum and B. juncea) exhibited also the presence of several unknown Se-species.     

The extraction and speciation of arsenic in rice flour by HPLC-ICP-MS

Several solvent mixtures and techniques for the extraction of arsenic (As) species from rice flour samples prior to their analysis by HPLC-ICP-MS were investigated. Microwave-assisted extraction using water at 80 °C for 30 min provided the highest extraction efficiency. Total recoveries of extracted As species were in good agreement with the total As concentrations determined by ICP-MS after microwave-assisted acid digestion of the samples. Arsenite [As(III)], arsenate [As(V)] and dimethylarsinic acid (DMAA) were the main species detected in rice flour samples.     

Inorganic speciation of As(III, V), Se(IV, VI) and Sb(III, V) in natural water with GF-AAS using solid phase extraction technology

The paper presents a procedure for the multi-element inorganic speciation of As(III, V), Se(IV, VI) and Sb(III, V) in natural water with GF-AAS using solid phase extraction technology. Total As(III, V), Se(IV, VI) and Sb(III, V) were determined according to the following procedure: titanium dioxide (TiO₂) was used to adsorb inorganic species of As, Se and Sb in sample solution; after filtration, the solid phase was prepared to be slurry for determination. For As(III), Se(IV) and Sb(III), their inorganic species were coprecipitated with Pb-PDC, dissolved in dilute nitric acid, and then determined. The concentrations of As(V), Se(VI) and Sb(V) can be calculated by the difference of the concentrations obtained by the above determinations. For the determination of As(III), Se(IV) and Sb(III), palladium was chosen as a modifier and pyrolysis temperature was 800 °C. Optimum conditions for the coprecipitation were listed for 100 ml of sample solution: pH 3.0, 15 min of stirring time, 40.0 μg l⁻¹ Pb(NO₃)₂ and 150.0 μg l⁻¹ APDC. The proposed method was applied to the determination of trace amounts of As(III, V), Se(IV, VI) and Sb(III, V) in river water and seawater.     

Approach for rapid extraction and speciation of mercury using a microtip ultrasonic probe followed by LC-ICP-MS

A fast method for mercury extraction from biological samples based on the use of HCl leaching plus different enzymatic hydrolysis (with and without mercury complexing agents), and the use of focussed ultrasounds (2-mm microtip) is here proposed. Total mercury content in several biological samples was determined by FI-ICP-MS using a carrier solution consisting of 0.1% (v/v) HCl, 0.1% (v/v) 2-mercaptoethanol, to avoid memory effect, and 0.15% (w/v) KCl. For mercury speciation a RP18 chromatographic column coupled to ICP-MS was used. A mobile phase consisting of 0.1% (v/v) formic acid, 0.1% (v/v) HFBA, 2% (v/v) methanol, and 0.02% (w/v) mM l-cysteine at pH 2.1 was used for chromatographic separation of the mercury species in the sample extracts. Extraction procedures were validated by using 50 mg of tuna fish tissue CRM-463 (2.85 ± 0.16 mg kg⁻¹ for methylmercury). The recoveries obtained were 99 ± 3% and 93 ± 1% after acid leaching (HCl 7 M) and enzymatic extraction (15 mg protease type XIV in 2.5% (v/v) 2-mercaptoethanol), respectively. The optimal sonication conditions (5 min of exposure time and 40% of ultrasound amplitude) were applied to 5 mg of CRM-463 (88 ± 5%), 5 mg of mussel tissue (81 ± 11%) and to 2 mg of zebra fish embryos (90 ± 10%) obtaining good recoveries in all cases. Methylmecury was found to be the most abundant Hg specie in all samples. The developed method is simple and rapid (5 min sample treatment); it is suitable for very small samples and does not alter the original form of the mercury species. Thus, it is of special interest in those cases in which validation of the results may often be hampered by lack of sample availability.     

Fabric phase sorptive extraction: An innovative sample preparation approach applied to the analysis of specific migration from food packaging

Additives added to food packaging materials can migrate to food in contact with them during storage and shelf life. A novel simple, fast and sensitive analyte extraction method based on fabric phase sorptive extraction (FPSE), followed by analysis using ultra-high performance liquid chromatography and mass spectrometry detection (UPLC-MS) was applied to the analysis of 18 common non-volatile plastic additives. Three FPSE media coated with different sol-gel sorbents characterized with different polarities including sol-gel poly(dimethylsiloxane), sol-gel poly(ethylene glycol) and sol-gel poly(tetrahydrofuran) were studied. All three FPSE media showed very satisfactory results. In general, compounds with low logP values seemed to have higher enrichment factors (EFs), especially with poly(tetrahydrofuran) and poly(ethylene glycol) media. For compounds with high logP values, the use of sol-gel poly(dimethylsiloxane) improved the enrichment capacity. Sample preparation time was optimized at 20 min for sample extraction and 10 min for solvent desorption. Acetonitrile was selected as desorption solvent since recoveries were over 70% for 13 out of 18 selected compounds in all FPSE media. The best extraction recovery values were obtained when compounds were dissolved in aqueous acetic acid solution (3%), where 17 out of 18 compounds showed improvement in their signal intensity after FPSE extraction and 10 obtained enrichment factors above 3 for all the tested FPSE media. When FPSE extracts were concentrated under nitrogen, 11 out of 18 compounds reached EFs values above 100.     

Toward use of a nano layered double hydroxide/ammonium pyrrolidine dithiocarbamate in speciation analysis: One-step dispersive solid-phase extraction of chromium species in human biological samples

Chromium is a controversial element with an important essentiality and toxicity. Depending on its different species, its speciation analysis in bio-origin matrices is of utmost importance. Ammonium pyrrolidine dithiocarbamate (APDC) and layered double hydroxide (LDH) nanoparticles, with the purpose of combining their outstanding performances, were served to speciate chromium ions in human biological samples. The as-obtained sorbent (nano LDH-APDC) - after characterization by X-ray diffraction (XRD), Fourier transform infrared (FT-IR) spectroscopy, thermal gravimetric analysis (TGA), and scanning electron microscopy (SEM) - was used as a novel pH-sensitive adsorbent in an integrated one-step dispersive solid-phase extraction (I-OS-DSPE), which combines the benefits of the air-assisted microextraction and dispersive solid-phase extraction methods. An interesting feature of the nano LDH-APDC sorbent is that it is dissolved in an aqueous solution when the pH of the solution is lower than 4. Thus the analyte elution step, as required in most of the sorbent-based extraction methods, was obviated by dissolving the sorbent in an acidic solution after extraction and separation from the sample solution. The Cr(VI) ions were first extracted, while the Cr(III) ions remained in the aqueous solution. The extract was then directly injected into a flame atomic absorption spectrometer with a micro-sampling introduction system, and the concentration of the Cr(III) ions was calculated by its subtraction from the total chromium ions present. Several variables including the pH (5), type and amount of the nanosorbent used (30 mg of nano (Zn-Al) LDH-APDC), number of extraction cycles (15 times), and elution conditions (200 µL of 6.0 mol L⁻¹ HNO₃) were investigated to achieve the maximum extraction efficiency. Under the optimum experimental conditions, the limit of detection, linear range, consumptive index, and enrichment factor for the Cr(VI) ions were 2.4 μg L⁻¹, 8.0–640 μg L⁻¹, 0.24, and 42.5 ± 1, respectively. These findings suggested that nano (Zn-Al) LDH-APDC could be regarded as a promising adsorbent for an efficient speciation of the chromium species in the human hair, nail, saliva, plasma, and urine samples.     

微波辅助萃取-液质联用技术测底泥砷、硒的化学形态

建立了用反相离子对色谱和电感耦合等离子体质谱的联用技术同时测定As（Ⅲ）、 As（Ⅴ）、 MMA、 DMA、 Se（Ⅳ）、 Se（Ⅵ）、 SeMet和SeCys的砷、硒化学形态分析方法. 分别从流动相pH值、离子对试剂的浓度、甲醇量和流速4个方面进行了分离测定条件的优化. 利用碰撞池技术（CCT）较好地解决了^40Ar^35Cl^＋复合离子对^75As的干扰, 并使^80Se的测定成为可能, 有效地提高了灵敏度. 将该方法应用于上海市苏州河底泥样品的微波辅助萃取液的形态分析中, 砷和硒的检出限分别达到0.4～1.3 和0.5～1.9 μg/L.     

Blank values, adsorption, pre-concentration, and sample preservation for arsenic speciation of environmental water samples

Arsenic is the focus of public attention because of its toxicity. Arsenic analysis, its toxicity, and its fate in the environment have been broadly studied, still its blank values, adsorption to sampling materials and pre-concentration of water samples as well as stabilization of arsenic compounds in water samples under field conditions have been very little investigated. In this study, we investigate the blank values and adsorption of arsenic compounds for different laboratory materials. We focused our work onto pre-concentration of water samples and how to stabilize arsenic compounds under field conditions. When using glassware for arsenic analysis, we suggest testing arsenic blank values due to the potential release of arsenic from the glass. Adsorption of arsenic compounds on different laboratory materials (<10%) showed little influence on the arsenic speciation. Pre-concentration of methanol-water solutions could result in potential overestimation of arsenic compounds concentrations. Successful pre-concentration of water samples by nitrogen-purge provides an analytical possibility for arsenic compounds with high recoveries (>80%) and low transformation of arsenic compounds. Thus, concentrations as low as 1 ng As l⁻¹ can be determined. Addition of ethylenediaminetetraacetic acid (EDTA) and storage in the dark can decrease the transformation among arsenic compounds in rainwater and soil-pore water for at least a week under field conditions.     

Trends in speciation analysis of vanadium in environmental samples and biological fluids--a review

A comprehensive review is presented addressing recent trends in the speciation and determination of vanadium in environmental and biological sample matrices, including important analytical aspects such as sample clean up, pre-concentration and method development. Methodology based on both separation and spectroscopic techniques for the determination of vanadium speciation is discussed. A brief outline of analytical principles, together with an overview of the recent developments and applications of vanadium speciation determination is included. The newer methods for detecting metal ions including hyphenated spectroscopic techniques and sample preparation schemes are also discussed.     

Extraction and speciation of arsenic in plants grown on arsenic contaminated soils

A sequential arsenic extraction method was developed that yielded extraction efficiencies (EE) that were approximately double those using current methods for terrestrial plants. The method was applied to plants from two arsenic contaminated sites and showed potential for risk assessment studies. In the method, plants were extracted first by 1:1 water-methanol followed by 0.1 M hydrochloric (HCl) acid. Total arsenic in plant and soil samples collected from contaminated sites was mineralized by acid digestion and detected by inductively coupled plasma-atomic emission spectrometry (ICP-AES) and hydride generation-atomic absorption spectrometry (HG-AAS). Arsenic speciation was done by high performance liquid chromatography coupled with HG-AAS (HPLC-HGAAS) and by HPLC coupled with ICP-mass spectrometry (HPLC-ICP-MS). Spike recovery experiments with arsenite (As(III)), arsenate (As(V)), methylarsonic acid (MA) and dimethylarsinic acid (DMA) showed stability of the species in the extraction processes. Speciation analysis by X-ray absorption near edge spectroscopy (XANES) demonstrated that no transformation of As(III) and As(V) occurred due to sample handling. Dilute HCl was efficient in extracting arsenic from plants; however, extraction and determination of organic species were difficult in this medium. Sequential extraction with 1:1 water-methanol followed by 0.1 M-HCl was most useful in extracting and speciating both organic and inorganic arsenic from plants. Trace amounts of MA and DMA in plants could be detected by HPLC-HGAAS aided by the process of separation and preconcentration of the sequential extraction method. Both organic and inorganic arsenic compounds could be detected simultaneously in synthetic gastric fluid extracts (GFE) but EEs by this method were lower than those of the sequential method. The developed sequential method was shown to be reliable and applicable to various terrestrial plants for arsenic extraction and speciation.