Arsenic speciation based on ion exchange high-performance liquid chromatography hyphenated with hydride generation atomic fluorescence and on-line UV photo oxidation

An on-line method capable of the separation of arsenic species was developed for the speciation of arsenite As(III), arsenate As(V), monomethylarsenic (MMA) and dimethylarsenic acid (DMA) in biological samples. The method is based on the combination of high-performance liquid chromatograph (HPLC) for separation, UV photo oxidation for sample digestion and hydride generation atomic fluorescence spectrometry (HGAFS) for sensitive detection. The best separation results were obtained with an anion-exchange AS11 column protected by an AG11 guard column, and gradient elution with NaH₂PO₄ and water as mobile phase. The on-line UV photo oxidation with 1.5% K₂S₂O₈ in 0.2 mol L^–1 NaOH in an 8 m PTFE coil for 40 s ensures the digestion of organoarsenic compounds. Detection limits for the four species were in the range of 0.11–0.15 ng (20 μL injected). Procedures were validated by analysis of the certified reference materials GBW09103 freeze-dried human urine and the results were in good agreement with the certified values of total arsenic concentration. The method has been successfully applied to speciation studies of blood arsenic species with no need of sample pretreatment. Speciation of arsenic in blood samples collected from two patients after the ingestion of realgar-containing drug reveals slight increase of arsenite and DMA, resulting from the digestion of realgar.     

Arsenic speciation based on ion exchange high-performance liquid chromatography hyphenated with hydride generation atomic fluorescence and on-line UV photo oxidation

An on-line method capable of the separation of arsenic species was developed for the speciation of arsenite As(III), arsenate As(V), monomethylarsenic (MMA) and dimethylarsenic acid (DMA) in biological samples. The method is based on the combination of high-performance liquid chromatograph (HPLC) for separation, UV photo oxidation for sample digestion and hydride generation atomic fluorescence spectrometry (HGAFS) for sensitive detection. The best separation results were obtained with an anion-exchange AS11 column protected by an AG11 guard column, and gradient elution with NaH2PO4 and water as mobile phase. The on-line UV photo oxidation with 1.5% K2S2O8 in 0.2 mol L(-1) NaOH in an 8 m PTFE coil for 40 s ensures the digestion of organoarsenic compounds. Detection limits for the four species were in the range of 0.11-0.15 ng (20 microL injected). Procedures were validated by analysis of the certified reference materials GBW09103 freeze-dried human urine and the results were in good agreement with the certified values of total arsenic concentration. The method has been successfully applied to speciation studies of blood arsenic species with no need of sample pretreatment. Speciation of arsenic in blood samples collected from two patients after the ingestion of realgar-containing drug reveals slight increase of arsenite and DMA, resulting from the digestion of realgar.     

Rapid separation of elemental species by multicapillary GC

Multicapillary gas chromatography has been applied to the speciation of organomercury compounds. Basic investigation of the fundamental properties of multicapillary columns, to evaluate their potential and limitations as a rapid separation unit, are presented. For analysis of methylated and ethylated mercury compounds a complete separation can be performed within 45 s under isothermal conditions. The adaptation of the technique for use with a purge and trap system and with an element-selective plasma-emission detector results in a compact and effective system for mercury speciation. Results from analysis of certified reference materials were in good agreement with certified values within the significance levels.     

Feasibility of Separation and Quantification of Inorganic Arsenic Species Using Ion-Exchange Membranes and Laser-Induced Breakdown Spectroscopy

Analytical methods for the determination of inorganic arsenic species have attracted much attention due to the high toxicity of these compounds and related legislative regulations for food. A new method for the separation and quantitation of As(III) and As(V) was developed using ion-exchange membranes and laser-induced breakdown spectroscopy (LIBS). Using the anion-exchange polymer membrane, As(V) was selectively collected on the membrane, and As(III) was filtered through the membrane. The separated As(V) on the membrane was directly determined by LIBS. The As(III) in the filtrate was subsequently oxidized to As(V) and collected by the membrane for LIBS analysis. The detection limit for As(V) was estimated to be 10?mg/kg. The recovery efficiencies for the arsenic species as standards were in the range of 97–99%. This method was applied for the analysis As-spiked water certified reference materials, and the results showed that the recovery for As(V) was 98.9%. This new speciation method is cost-effective, simple, and low labor-intensive for the quantitation of inorganic arsenic.     

Determination of arsenic species in marine samples by HPLC-ICP-MS.

Arsenic speciation analysis in marine samples was performed using high performance liquid chromatography (HPLC) with ICP-MS detection. The separation of eight arsenic species viz. arsenite (As(III)), monomethylarsonic acid (MMA), dimethylarsinic acid (DMA), arsenate (As(V)), arsenobetaine, trimethylarsine oxide (TMAO), arsenocholine and tetramethylarsonium ion (TeMAs) was achieved on a Shiseido Capcell Pak C18 column by using an isocratic eluent (pH 3.0), in which condition As(III) and MMA were co-eluted. The entire separation was accomplished in 15 min. The detection limits for 8 arsenic species by HPLC/ICP-MS were in the range of 0.02 - 0.10 microg L(-1) based on 3sigma of blank response (n=9). The precision was calculated to be 3.1-7.3% (RSD) for all eight species. The method then successfully applied to several marine samples e.g., oyster, scallop, fish, and shrimps. For the extraction of arsenic species from seafood products, the low power microwave digestion was employed. The extraction efficiency was in the range of 52.9 - 112.3%. Total arsenic concentrations were analyzed by using the microwave acid digestion. The total arsenics in the certified reference materials (DORM-2 and TORT-2) were analyzed and agreed with the certified values. The concentrations of arsenics in marine samples were in the range 6.6 - 35.1 microg g(-1).     

Analytical methodology for speciation of arsenic in environmental and biological samples

A literature search on the speciation of arsenic in environmental and biological samples shows an increasing interest of many researchers in the subject. Because of the low level of arsenic species in real samples, many problems related with its speciation remain unresolved: species instability during sampling, storage and sample treatment, incomplete recovery of all species, matrix interferences, lack of appropriate certified reference materials and of sensitive analytical methods, etc. These aspects are underlined in this paper. The continued development of new analytical procedures pretending to solve some of these problems claim for an up-to-date knowledge of the recent publications. Therefore, this paper pretends to review the latest publications on the chemical speciation of arsenic, emphasizing the increasing activity in the development of accurate and precise analytical methods. In most of the cases, separation and preconcentration is necessary, followed by element-specific detection for sensitivity improvement. Hydride generation following separation procedures (e.g., ion-exchange or high performance liquid chromatography) coupled to atomic absorption or atomic emission detectors proved to have sufficient sensitivity to monitor arsenic exposure, although restricts the analysis to hydride-forming species. Modified procedures including some kind of heating in the presence of highly oxidizing agents have proved successful to completely decompose the arsenic containing compounds to arsenate and so to extend the range of compounds which can be determined by these methods. On-line arrangements have the additional advantage of avoiding excessive sample handling, although some of them involve numerous steps and others are too costly to be recommended for routine use. The analytical figures of merits, specially detection limits are given for most of the methods in order to afford comparison and judge possible applicability. These studies, which have been approached in many different ways, would lead to knowledge that are determinant in the understanding of the cycle of this element in environment and of its physiological and toxicological behavior in the living organisms.     

NIES certified reference materials for arsenic speciation

 The National Institute for Environmental Studies (NIES) recently prepared two candidate certified reference materials (CRMs) for arsenicals to meet the growing demand for the quality assurance of arsenic speciation analysis. The NIES candidate CRM No. 14 Brown Alga was prepared from Hijiki seaweed for the certification of inorganic arsenic content, and No. 15 Scallop was prepared from adductor muscle of scallop for the certification of arsenobetaine content. The preparation of the candidate CRMs is briefly described. Cooperative analyses for total arsenic content of the candidate CRMs have been underway. The preliminary speciation analysis at NIES revealed difficulty in establishing suitable conditions for extracting arsenic species from the materials. Chromatograms of arsenic species by a high performance liquid chromatography-inductively coupled plasma mass spectrometric detection system are presented to provide information about arsenic species present in these candidate CRMs.     

Arsenic speciation in contaminated soils

A method for arsenic speciation in soils is developed, based on extraction with a mixture of 1 mol l(-1) of phosphoric acid and 0.1 mol l(-1) of ascorbic acid, and further measurement with the coupling liquid chromatography (LC)-ultraviolet (UV) irradiation-hydride generation (HG)-inductively coupled plasma mass spectrometry (ICP/MS). The stability of the arsenic species in the extracts is also studied. The speciation method applied to several Spanish agricultural contaminated soils from the Aznalcollar zone shows that arsenate is the main species in all the soils analysed and that in some samples arsenite and methylated species could also be detected. The determination of the "pseudototal" arsenic in these soils, obtained by applying extraction with aqua regia (ISO Standard 11466), is also carried out. Both the speciation method and the aqua regia method are applied to several certified reference materials (CRMs) in which total arsenic content is certified. Finally, the same LC-UV-HG coupling with atomic fluorescence spectrometry (AFS) detection reveals to be a valid coupling system to perform arsenic speciation in the soils according to its fair quality parameters and easy utilisation.     

Determination of inorganic arsenic species in natural waters—Benefits of separation and preconcentration on ion exchange and hybrid resins

A simple method for the separation and determination of inorganic arsenic (iAs) species in natural and drinking water was developed. Procedures for sample preparation, separation of As(III) and As(V) species and preconcentration of the total iAs on fixed bed columns were defined. Two resins, a strong base anion exchange (SBAE) resin and a hybrid (HY) resin were utilized. The inductively-coupled plasma-mass spectrometry method was applied as the analytical method for the determination of the arsenic concentration in water. The governing factors for the ion exchange/sorption of arsenic on resins in a batch and a fixed bed flow system were analyzed and compared. Acidity of the water, which plays an important role in the control of the ionic or molecular forms of arsenic species, was beneficial for the separation; by adjusting the pH values to less than 8.00, the SBAE resin separated As(V) from As(III) in water by retaining As(V) and allowing As(III) to pass through. The sorption activity of the hydrated iron oxide particles integrated into the HY resin was beneficial for bonding of all iAs species over a wide range of pH values from 5.00 to 11.00. The resin capacities were calculated according to the breakthrough points in a fixed bed flow system. At pH 7.50, the SBAE resin bound more than 370 μg g⁻¹ of As(V) while the HY resin bound more than 4150 μg g⁻¹ of As(III) and more than 3500 μg g⁻¹ of As(V). The high capacities and selectivity of the resins were considered as advantageous for the development and application of two procedures, one for the separation and determination of As(III) (with SBAE) and the other for the preconcentration and determination of the total arsenic (with HY resin). Methods were established through basic analytical procedures (with external standards, certified reference materials and the standard addition method) and by the parallel analysis of some samples using the atomic absorption spectrometry-hydride generation technique. The analytical properties of both procedures were similar: the limit of detection was 0.24 μg L⁻¹, the limit of quantification was 0.80 μg L⁻¹ and the relative standard deviations for samples with a content of arsenic from 10.00 to 300.0 μg L⁻¹ ranged from 1.1 to 5.8%. The interference effects of anions commonly found in water and some organic species which can be present in water were found to be negligible. Verification with certified reference materials proved that the experimental concentrations found for model solutions and real samples were in agreement with the certified values.     

Arsenic species in certified reference material MURST-ISS-A2 (Antarctic krill)

Arsenic compounds were quantified in the certified reference material MURST-ISS-A2 (Antarctic krill) using HPLC/ICPMS. The data should prove useful for assessing the accuracy of arsenic speciation procedures.     

Speciation of arsenic in chicken meat by anion-exchange liquid chromatography with inductively coupled plasma-mass spectrometry

A method was developed for speciation analysis of arsenic in chicken meat. Different procedures were optimized for the recovery of arsenic compounds without destroying the original compounds, and 2 anion-exchange liquid chromatography columns were compared for the separation of arsenic species prior to on-line detection by inductively coupled plasma-mass spectrometry. The 2 species found were dimethylarsinic acid (106 +/- 5 ng/g) and arsenobetaine (37 +/- 4 ng/g). The stability of arsenic species in a chicken meat candidate reference material for at least 12 months was demonstrated.     

Determination of arsenic compounds in beverages by high-performance liquid chromatography-inductively coupled plasma mass spectrometry

Arsenic compounds including arsenous acid (As(III)), arsenic acid (As(V)), dimethylarsinic acid (DMA) and monomethylarsonic acid (MMA) were separated by high-performance liquid chromatography (HPLC) and detected by inductively coupled plasma mass spectrometry (ICP-MS). A Hamilton PRX-100 anionic-exchange column and a pH 8.5 K₂HPO₄/KH₂PO₄ 5.0 × 10⁻³ mol L⁻¹ mobile phase were used to achieve arsenic speciation. The separation of arsenic species provided peaks of As(III) at 2.75 min, DMA at 3.33 min, MMA at 5.17 min and As(V) at 12.5 min. The detection limits, defined as three times the standard deviation of the lowest standard measurements, were found to be 0.2, 0.2, 0.3 and 0.5 ng mL⁻¹ for As(III), DMA, MMA and As(V), respectively. The relative standard deviation values for a solution containing 5.0 μg L⁻¹ of As(III), DMA, MMA and As(V) were 1.2, 2.1, 2.5 and 3.0%, respectively. This analytical procedure was applied to the speciation of arsenic compounds in drinking (soft drink, beer, juice) samples. The validation of the procedure was achieved through the analysis of arsenic compounds in water and sediment certified reference materials.     

High performance liquid chromatography hydride generation in situ trapping graphite furnace atomic absorption spectrometry: A new way of performing speciation analysis using GFAAS as detector

A new procedure for the speciation analysis of hydride forming elements using GFAAS as detector is proposed. The separation of the species is performed by HPLC and the eluent flow is merged with HCl and NaBH₄ solutions moved by peristaltic pumps controlled by a flow injection apparatus. As the species emerges from the column, its respective hydride is formed and carried through the autosampler capillary to an Ir treated graphite tube pre-heated at 300 °C, where it is trapped. After the hydride collection, the autosampler arm is moved from the tube and atomization takes place. The sequence is repeated for the next emerging species. The feasibility of the system was evaluated for the speciation of As (III) and As (V) in waste water samples. The retention times were previously determined using a more concentrated mixed analytical solution and a quartz tube as atomizer. The analytical curves obtained by the proposed procedure showed similar slopes for both species as well as coefficient of regression better than 0.99. Limits of detection were 0.2 ng/mL for both species, 50 times better then the same assembly using a quartz tube atomizer. In the analysis of certified reference materials the sum of the As (III) and As (V) species concentrations were in close agreement with the arsenic concentration certified for total arsenic.     

Arsenic speciation in marine product samples: Comparison of extraction-HPLC method and digestion-cryogenic trap method

For the arsenic speciation in marine product samples, two types of pretreatment-analysis combination were compared. One is the combination of solvent extraction and high performance liquid chromatography (HPLC) followed by a highly sensitive arsenic detection, while the other is the combination of alkaline digestion and cryogenic trap (CT) method followed by a highly sensitive arsenic detection. For six certified reference materials (CRMs) of marine animal samples, the concentrations of arsenobetaine (AsB) obtained from the extraction-HPLC method were very consistent with those of trimethylated arsenic species measured by the digestion-CT method. For four seaweed samples, the determination of three arsenosugars (Sugar-1, Sugar-2, and Sugar-3) was favorably carried out by the extraction-HPLC method. Those seaweed samples were also subjected to the digestion-CT method, and the amounts of dimethylated arsenic species measured by the method were approximately equal to the sum of the amounts of dimethylarsinic acid (DMAA) and three arsenosugars (Sugar-1 + Sugar-2 + Sugar-3) obtained from the extraction-HPLC method.     

Separation and Detection of Arsenic and Selenium Species in Environmental Samples by HPLC-ICP-MS

A method is presented for arsenic speciation analysis of an oyster sample using ion chromatography coupled with an inductively coupled plasma mass spectrometry (ICP-MS) instrument. A strong anion exchange resin was employed with a step gradient elution of 0.1 mM/0.1 M K 2 SO 4 at pH 10.2. Arsenobetaine and dimethylarsinic acid were determined following extraction based on trypsin enzymolysis with 95-100% extraction efficiency. Limits of detection in the range 0.1-0.3 mg kg m 1 of arsenic were obtained for organic arsenic species. No inorganic arsenic was detected. Validation was performed using TORT-2 as a certified reference material. Although high performance liquid chromatography (HPLC) coupled to ICP-MS is an effective method for speciation analysis it is not always necessary to obtain such a detailed picture. A simple liquid chromatographic separation technique based upon mini-column technology is presented. It was developed to obtain a fast, efficient and reliable separation of inorganic from organic, i.e. assumed toxic from non-toxic, arsenic and selenium species suitable for use as an initial screening method for environmental analysis. Two types of strong anion exchange resin were tested. Excellent separation was obtained for both min-column resins and analysis times were within 7 min. Limits of detection obtained for inorganic arsenic, organic arsenic, selenomethionine, Se IV and Se VI were 1.6, 1.8, 66, 32 and 22 µg kg m 1 , respectively.     

Speciation of arsenic compounds in fish and oyster tissues by capillary electrophoresis-inductively coupled plasma-mass spectrometry

A capillary electrophoresis-inductively coupled plasma-mass spectrometric (CE-ICP-MS) method for the speciation of six arsenic compounds, namely arsenite [As(III)], arsenate [As(V)], monomethylarsonic acid, dimethylarsinic acid, arsenobetaine and arsenocholine is described. The separation has been achieved on a 70 cm length x 75 microm ID fused-silica capillary. The electrophoretic buffer used was 15 mM Tris (pH 9.0) containing 15 mM sodium dodecyl sulfate (SDS), while the applied voltage was set at +22 kV. The arsenic species in biological tissues were extracted into 80% v/v methanol-water mixture, put in a closed centrifuge tube and kept in a water bath, using microwaves at 80 degrees C for 3 min. The extraction efficiencies of individual arsenic species added to the sample at 0.5 microg As/g level were between 96% and 107%, except for As(III), for which it was 89% and 77% for oyster and fish samples, respectively. The detection limits of the species studied were in the range 0.3-0.5 ng As/mL. The procedure has been applied for the speciation analysis of two reference materials, namely dogfish muscle tissue (NRCC DORM-2) and oyster tissue (NIST SRM 1566a), and two real-world samples.     

Low pressure chromatographic separation of inorganic arsenic species using solid phase extraction cartridges

Routine water analysis of arsenic species requires simple, inexpensive, rapid and sensitive methods. To this end, we have developed two methods, which are based on the use of inexpensive solid phase extraction (SPE) cartridges as low pressure chromatographic columns for separation and hydride generation atomic absorption spectrometry (HGAAS) and hydride generation atomic fluorescence spectrometry (HGAFS) for detection of arsenic. Both anion exchange and reverse phase cartridges were successfully used to separate arsenite [As(III)] and arsenate [As(V)]. The composition, concentration, and pH of eluting buffers and the effect of flow rate were systematically investigated. Speciation of inorganic As(III) and As(V) were achieved within 1.5 min, with detection limits of 0.2 and 0.4 ng/ml, respectively. Both isocratic and step gradient elution techniques were suitable for the baseline resolution of As(III) and As(V) using anion exchange cartridges. Application of the methods to the speciation of As(III) and As(V) in untreated water, tap water, and bottled water samples were demonstrated. Results from the speciation of arsenic in a standard reference material water sample using these methods were in good agreement with the certified value and with inter-laboratory comparison results obtained using HPLC separation and inductively coupled plasma mass spectrometric detection (HPLC-ICPMS).     

Ultrasensitive and Simultaneous Determination of Arsenic and Antimony in Clinical Samples by Atomic Fluorescence Spectrometry

The determination of trace elements in human fluids facilitates the identification of metabolic disorders and physiological abnormities in clinical diagnosis. Elemental concentrations in serum, urine, and saliva are often low and highly prone to contamination. Consequently, a simple and ultrasensitive detection technique is required. In this study, a method was developed for the simultaneous determination of trace arsenic and antimony in clinical samples by hydride generation atomic fluorescence spectrometry. The experimental parameters that affect the generation, delivery, and atomization of volatile arsenic and antimony hydrides were investigated. The limits of quantification were calculated to be 0.0037 nanogram per milliliter and 0.0070 nanogram per milliliter for arsenic and antimony, respectively. The method was successfully applied for the analysis of fortified human serum, urine, saliva, and certified reference materials. The results obtained by the reported method were not statistically different from the certified values at the 95 percent confidence level.     

A decomposition procedure for the determination of arsenic in marine samples

The use of wet and dry ashing procedures to decompose marine biological tissues and to degrade organoarsenic compounds to inorganic arsenic for analysis by zinc-column arsine generation and atomic-absorption spectrophotometry was investigated. Wet ashing with nitric, sulphuric and perchloric acids (10:2:3 v/v) released the largest percentage of arsenic from fish tissue and quantitatively degraded methylated and other organoarsenic compounds to inorganic arsenic. The arsenic concentrations found when standard reference materials were ashed with this acid mixture were in agreement with the certified values.     

Separation and determination of arsenic species in water by selective exchange and hybrid resins

A simple and efficient method for separation and determination of inorganic arsenic (iAs) and organic arsenic (oAs) in drinking, natural and wastewater was developed. If arsenic is present in water prevailing forms are inorganic acids of As(III) and As(V). oAs can be found in traces as monomethylarsenic acid, MMA(V), and dimethylarsenic acid, DMAs(V). Three types of resins: a strong base anion exchange (SBAE) and two hybrid (HY) resins: HY-Fe and HY-AgCl, based on the activity of hydrated iron oxides and a silver chloride were investigated. It was found that the sorption processes (ion exchange, adsorption and chemisorptions) of arsenic species on SBAE (ion exchange) and HY resins depend on pH values of water. The quantitative separation of molecular and ionic forms of iAs and oAs was achieved by SBAE and pH adjustment, the molecular form of As(III) that exists in the water at pH <8.0 was not bonded with SBAE, which was convenient for direct determination of As(III) concentration in the effluent. HY-Fe resin retained all arsenic species except DMAs(V), which makes possible direct measurements of this specie in the effluent. HY-AgCl resin retained all iAs which was convenient for direct determination of oAs species concentration in the effluent. The selective bonding of arsenic species on three types of resins makes possible the development of the procedure for measuring and calculation of all arsenic species in water. In order to determine capacity of resins the preliminary investigations were performed in batch system and fixed bed flow system. Resin capacities were calculated according to breakthrough points in a fixed bed flow system which is the first step in designing of solid phase extraction (SPE) module for arsenic speciation separation and determination. Arsenic adsorption behavior in the presence of impurities showed tolerance with the respect to potential interference of anionic compounds commonly found in natural water. Proposed method was established performing standard procedures: with external standard, certified reference material and standard addition method. Two analytical techniques: the inductively coupled plasma mass spectrometry (ICP-MS) and atomic absorption spectroscopy-hydride generation (AAS-GH) were comparatively applied for the determination of arsenic in all arsenic species in water. ICP-MS detection limit was 0.2 μg L⁻¹ and relative standard deviation (RSD) of all arsenic species investigated was between 3.5 and 5.1%.