Extraction of arsenic species from airborne particulate filters—Application to an industrial area of Greece

In the present study, the extraction of the arsenic species arsenite (As(III)), arsenate (As(V)), monomethyarsonic (MMA) and dimethylarsinic acid (DMA) from airborne particulate filters was investigated and optimized. For this purpose, total suspended particulate matter as well as size fractionated aerosol samples were collected from the industrial area of Aspropyrgos, Greece, in glass fibre and polycarbonated filters, respectively. Among H₃PO₄ and HCl, tested in various concentrations, concentrated HCl was found to be the most effective extractant for arsenic from both polycarbonated and glass fibre filters, without provoking any arsenic species transformation. However, the quantitative extraction of arsenic species from glass fibre filters required the subsequent washing of the filters with ultrapure water after their leaching with concentrated HCl. The developed procedure was applied to airborne particulate filters for arsenic speciation in Aspropyrgos' atmosphere. The results showed an enrichment of As in the fine (PM_2.5) compared with the coarse (PM_10–2.5) fraction of airborne particulates, while As(V) was found to be the predominant arsenic species in all samples. Finally, As concentration in the PM₁₀ fraction, for the investigated area and time period from December 2004 to June 2006, was below the target value of 6 ng As m^− 3, referred in the Directive 2004/107 of European Union.     

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.     

Development of an analytical approach for determination of total arsenic and arsenic (III) in airborne particulate matter by slurry sampling and HG-FAAS

Slurry sampling (SS) with hydride generation atomic absorption spectrometry (HG-AAS) was used to analyze 3 particulate matter samples collected in the Bananeira Village, Brazil, in 2005. The relative standard deviation (RSD), used to assess the precision, was lower than 4.8%. The accuracy of this method was confirmed by the analysis of certified atmospheric particulate matter urban dust reference material SRM 1649a. This method (SS/HG-AAS) was used to determine total arsenic and arsenic (III) in three particulate matter samples. In these samples, the total arsenic concentrations varied from 3.8 to 20.0 ng m^− 3, while As (III) concentrations varied from 2.7 to 10.5 ng m^− 3. All samples were also analyzed using acid digestion in digest block with cold finger and detection for HG-AAS. A paired t-test demonstrated no significant difference (95% CL) between the results obtained using these two sample preparation procedures. The limit of quantification, calculated considering the mass of particulate matter collected on every filter, was 0.6 ng m^− 3 for As total and 1.0 ng m^− 3 for As (III).     

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.     

Determination of total inorganic arsenic in water using on-line pre-concentration and hydride-generation atomic absorption spectrometry

A rapid and sensitive method for the on-line separation and pre-concentration of inorganic arsenic in water samples is described. The analyte in the pentavalent oxidation state is reduced to its trivalent form with l-cysteine and the total inorganic arsenic is sorbed onto activated alumina in the acid form in a mini-column coupled to a FI-HG AAS system. Afterwards, it is eluted with 3 mol l⁻¹ HCl. An enrichment factor of 7 was obtained, allowing an analytical flow rate of about 28 determinations per hour. The limits of detection (3σ) and of quantification (10σ) were calculated as LOD = 0.15 μg l⁻¹ of As and LOQ = 0.5 μg l⁻¹ of As, respectively. Relative standard deviations (n = 10) less than 8% were obtained for different arsenic concentrations and the accuracy was verified by analysing certified reference materials. Different kinds of samples, such as mineral water, drinking water, river water and natural spring water were analyzed and good agreement was obtained with the values from spiked experiments.     

Determination of total arsenic and arsenic (III) in phosphate fertilizers and phosphate rocks by HG-AAS after multivariate optimization based on Box-Behnken design

In the present paper, a procedure for the determination of total arsenic and arsenic (III) in phosphate fertilizers and phosphate rocks by slurry sampling (SS) with hydride generation atomic absorption spectrometry (HG-AAS) is proposed. Arsenic (III) is determinated directly and total arsenic is determinated after reduction reaction. The procedure was optimized for the flow rate of NaBH₄, NaBH₄ and hydrochloric acid concentrations using a full two-level factorial and also a Box-Behnken design. Slurry preparation with hydrochloric acid in an ultrasonic bath allowed the determination of arsenic (III) with limits of detection and quantification of 0.1 and 0.3 μg L⁻¹, respectively. The precision of results, expressed as relative standard deviation (RSD), was always lower than 3%. The accuracy of this method was confirmed by analysis of certified sediment reference materials, while the procedure also allows for calibration using aqueous external standards. This method (SS/HG-AAS) was used to determine total arsenic and arsenic (III) in two phosphate rock samples and two phosphate fertilizer samples. In these samples, total arsenic concentrations varied from 5.2 to 20.0 mg kg⁻¹, while As (III) concentrations varied from 2.1 to 5.5 mg kg⁻¹, in agreement with published values. All samples were also analyzed using acid digestion/HG-AAS. Both, a paired t-test and a linear regression model demonstrated no significant difference (95% CL) between the results obtained using these two sample preparation procedures.     

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.     

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.     

Optimization of a GFAAS method for determination of total inorganic arsenic in drinking water

The new 10 μg l⁻¹ arsenic standard in drinking water has been a spur to the search for reliable routine analytical methods with a limit of detection at the μg l⁻¹ level. These methods also need to be easy to handle due to the routine analyses that are required in drinking water monitoring. Graphite furnace atomic absorption spectrometry (GFAAS) meets these requirements, but the limit of detection is generally too high except for methods using a pre-concentration or separation step. The use of a high-intensity boosted discharge hollow-cathode lamp decreases the baseline noise level and therefore allows a lower limit of detection. The temperature program, chemical matrix modifier and thermal stabilizer additives were optimized for total inorganic arsenic determination with GFAAS, without preliminary treatment. The optimal furnace program was validated with a proprietary software. The limit of detection was 0.26 μg As l⁻¹ for a sample volume of 16 μl corresponding to 4.2 pg As. This attractive technique is rapid as 20 samples can be analysed per hour. This method was validated with arsenic reference solutions. Its applicability was verified with artificial and natural groundwaters. Recoveries from 91 to 105% with relative standard deviation <5% can be easily achieved. The effect of interfering anions and cations commonly found in groundwater was studied. Only phosphates and silicates (respectively at 4 and 20 mg l⁻¹) lead to significant interferences in the determination of total inorganic arsenic at 4 μg l⁻¹.     

A microwave-assisted sequential extraction of water and dilute acid soluble arsenic species from marine plant and animal tissues

This paper describes the use of dilute nitric acid for the extraction and quantification of arsenic species. A number of extractants (e.g. water, 1.5 M orthophosphoric acid, methanol-water and dilute nitric acid) were tested for the extraction of arsenic from marine biological samples, such as plants that have proved difficult to quantitatively extract. Dilute 2% (v/v) nitric acid was found to give the highest recoveries of arsenic overall and was chosen for further optimisation. The optimal extraction conditions for arsenic were 2% (v/v) HNO₃, 6 min⁻¹, 90 °C. Arsenic species were found to be stable under the optimised conditions with the exception of the arsenoriboses which degraded to a product eluting at the same retention time as glycerol arsenoribose. Good agreement was found between the 2% (v/v) HNO₃ extraction and the methanol-water extraction for the certified reference material DORM-2 (AB 17.1 and 16.2 μg g⁻¹, respectively, and TETRA 0.27 and 0.25 μg g⁻¹, respectively), which were in close agreement with the certified concentrations of AB 16.4 ± 1.1 μg g⁻¹ and TETRA 0.248 ± 0.054 μg g⁻¹.To preserve the integrity of arsenic species, a sequential extraction technique was developed where the previously methanol-water extracted pellet was further extracted with 2% (v/v) HNO₃ under the optimised conditions. Increases in arsenic recoveries between 13% and 36% were found and speciation of this faction revealed that only inorganic and simple methylated species were extracted.     

Arsenic speciation in edible alga samples by microwave-assisted extraction and high performance liquid chromatography coupled to atomic fluorescence spectrometry

Twelve commercially available edible marine algae from France, Japan and Spain and the certified reference material (CRM) NIES No. 9 Sargassum fulvellum were analyzed for total arsenic and arsenic species. Total arsenic concentrations were determined by inductively coupled plasma atomic emission spectrometry (ICP-AES) after microwave digestion and ranged from 23 to 126 μg g⁻¹. Arsenic species in alga samples were extracted with deionized water by microwave-assisted extraction and showed extraction efficiencies from 49 to 98%, in terms of total arsenic. The presence of eleven arsenic species was studied by high performance liquid chromatography–ultraviolet photo-oxidation–hydride generation atomic–fluorescence spectrometry (HPLC–(UV)–HG–AFS) developed methods, using both anion and cation exchange chromatography. Glycerol and phosphate sugars were found in all alga samples analyzed, at concentrations between 0.11 and 22 μg g⁻¹, whereas sulfonate and sulfate sugars were only detected in three of them (0.6-7.2 μg g⁻¹). Regarding arsenic toxic species, low concentration levels of dimethylarsinic acid (DMA) (<0.9 μg g⁻¹) and generally high arsenate (As(V)) concentrations (up to 77 μg g⁻¹) were found in most of the algae studied. The results obtained are of interest to highlight the need to perform speciation analysis and to introduce appropriate legislation to limit toxic arsenic species content in these food products.     

Hemimicelle capped functionalized carbon nanotubes-based nanosized solid-phase extraction of arsenic from environmental water samples

The end functionalization of CNTs can introduce oxygen-containing negatively functional groups such as -COOH, -OH, or -CO on their surface site. If cationic surfactant such as cetyltrimethylammonium chloride (CTAC) was added to the functionalized CNTs, then interactions such as hydrophobic and ionic may lead to formation of hemimicelle/admicelle aggregates on the CNTs, a new kind of adsorbents, namely, the hemimicelle capped CMMWCNTs, is obtained. The application of the hemimicelle capped carbon nanotubes-based nanosized solid-phase extraction (SPE) adsorbents in environmental analysis is reported for the first time using arsenic as model target. The effect of adsorption and desorption conditions for arsenic including the amount of surfactant, initial pH of sample solution, the ultrasonic time of sample solution, the amount of electrolyte, flow rate, eluent and its amount were investigated and optimized prior to its determination by atomic fluorescence spectrophotometry (AFS). Arsenic can be quantitatively retained on the hemimicelle capped CMMWCNTs at pH 5-6 from sample volume up to 500 mL and then eluted completely with 2 mol L⁻¹ HNO₃ in the presence of 10 mg L⁻¹ CTAC. The method detection limit for arsenic determination with AFS detection was 2 ng L⁻¹, and the relative standard deviation (RSD, n = 11) was 5.3% at the 0.5 μg L⁻¹ level. The recoveries of arsenic in the spiked environmental water samples ranged from 94% to 104.29% with 500 mL of water sample. The proposed method has been applied successfully to the analysis of arsenic in aqueous environmental samples, which demonstrates the hemimicelle capped CMMWCNTs can be an excellent SPE adsorbents for arsenic pretreatment and enrichment from real water samples.     

Application of arsenic to electrophotoreceptors

Arsenic has been applied to many electronic devices such as electrophotoreceptors, gallium arsenide (GaAs) semiconductors and solid-state image pickup devices. For electrophotoreceptors selenium–arsenic (Se? As) alloys are coated onto the conductive substrate of the receptors. Arsenic is mostly used in electophotoreceptors in electronic devices. During the coating process, a part of the gaseous arsenic is released through an exhaust system. In order to avoid arsenic being discharged to the atmosphere, bag filters and high-efficiency particulate air filters are set before the exhaust port. Any arsenic which still exists in the waste water after washing tools and jigs from the coating process is collected by sedimentation before discharging. The Ames salmonella/microsome plate test for As₂Se₃ indicated no mutagenic activity under the test system used. For the safety of workers engaged in arsenic-related jobs, they received a medical examination once every six months. No negative trends from the examination was found in 428 men who received the examination from Autumn 1980 to Spring 1987.     

Determination of total arsenic and toxicologically relevant arsenic species in fish by using electrothermal and hydride generation atomic absorption spectrometry

A scheme for the determination of total As by electrothermal atomic absorption spectrometry (ETAAS) and the sum of toxicologically relevant arsenic species (As(III), As(V), monomethylarsonate (MMA) and dimethylarsinate (DMA) using hydride generation AAS (HGAAS) in fish samples was developed. Simple and fast microwave assisted extraction in tetramethylammonium hydroxide (TMAH, 0.075% m / v) or in water-methanol mixture (80 + 20 v / v) for 20 min is proposed for quantitative leaching of arsenic species from fish tissue. Total As was measured by ETAAS directly in the TMAH extract under optimal instrumental parameters (pyrolysis temperature 1400 °C and atomization temperature 2000 °C) with Pd as modifier ensuring thermal stabilization and isoformation of all extracted arsenic species. The analytical features of the method are as follows: limit of detection (LOD) 0.45 μg g^− 1 (dry wt.), within-run and between-run precision in the range 4-8% and 5-12%, respectively, for arsenic contents 0.5-30 μg g^− 1 and recoveries 98-102%. The sum of toxicologically relevant arsenic species (As(III) + As(V) + MMA + DMA) was determined by flow injection HGAAS directly from the TMAH extract or water-methanol mixture and trapping of arsines onto Zr-Ir coated graphite tube followed by ETAAS measurement. l-cysteine is used as reagent for leveling off responses of different arsenic species in the presence of TMAH or water-methanol mixture. The LODs achieved are 0.0038 and 0.0031 μg g^− 1 (dry wt.), respectively, for fish extracts in TMAH and in water-methanol mixture. Within-batch and between-batch RSDs are in the range 3-5% and 4-7% for arsenic contents of 0.009-0.25 μg g^− 1 (dry wt.) for TMAH extracts and 2-4% and 3-6% for methanol water extracts, respectively. Selective reaction media for generation of respective hydrides from arsenic species were recommended for further speciation purposes in methanol-water extracts, viz. citrate buffer (pH 5.2) for the determination of As(III), 0.2 mol L^− 1 acetic acid for the determination of As(III) + DMA and 7 mol L^− 1 hydrochloric acid for the determination of inorganic As(III) + As(V). LODs are 0.0035, 0.0051 and 0.0046 μg g^− 1 (dry wt.) for As(III), DMA and As(V). The relative standard deviation is 4-8% for three arsenic species at As levels of 0.009-0.5 μg g^− 1 (dry wt.). The accuracy of the proposed speciation scheme is confirmed by the analysis of certified reference materials.     

Preservation of arsenic species in water samples using phosphoric acid--limitations and long-term stability

The preservation of arsenic species in water samples is an indispensable method to avoid their changes during storage, if it is not possible to analyse them immediately. The aim of this investigation was to demonstrate the limitations of the suggested method by using phosphoric acid as a preservation agent. The samples remain stable for 3 months, even if they show evidence of high concentrations of iron or manganese. Critical is an increasing pH > 3. Theoretically, a precipitation of strengite (Fe₃(PO₄)₂) could occur, which should be avoided. Phosphoric acid with a final concentration of 10 mM is recommended as a preservation agent, combined with keeping the samples cool (6 °C) and dark. Filtration of samples before preservation may be carried out with respect to the analytical aim to distinguish between the total and soluble fraction (without colloids). It was shown that filtered and non-filtered samples can be preserved by utilising the above mentioned scheme.     

Enzyme-assisted extraction and liquid chromatography mass spectrometry for the determination of arsenic species in chicken meat

Chicken is the most consumed meat in North America. Concentrations of arsenic in chicken range from μg kg⁻¹ to mg kg⁻¹. However, little is known about the speciation of arsenic in chicken meat. The objective of this research was to develop a method enabling determination of arsenic species in chicken breast muscle. We report here enzyme-enhanced extraction of arsenic species from chicken meat, separation using anion exchange chromatography (HPLC), and simultaneous detection with both inductively coupled plasma mass spectrometry (ICPMS) and electrospray ionization tandem mass spectrometry (ESIMS). We compared the extraction of arsenic species using several proteolytic enzymes: bromelain, papain, pepsin, proteinase K, and trypsin. With the use of papain-assisted extraction, 10 arsenic species were extracted and detected, as compared to 8 detectable arsenic species in the water/methanol extract. The overall extraction efficiency was also improved using a combination of ultrasonication and papain digestion, as compared to the conventional water/methanol extraction. Detection limits were in the range of 1.0–1.8 μg arsenic per kg chicken breast meat (dry weight) for seven arsenic species: arsenobetaine (AsB), inorganic arsenite (As^III), dimethylarsinic acid (DMA), monomethylarsonic acid (MMA), inorganic arsenate (As^V), 3-nitro-4-hydroxyphenylarsonic acid (Roxarsone), and N-acetyl-4-hydroxy-m-arsanilic acid (NAHAA). Analysis of breast meat samples from six chickens receiving feed containing Roxarsone showed the presence of (mean ± standard deviation μg kg⁻¹) AsB (107 ± 4), As^III (113 ± 7), As^V (7 ± 2), MMA (51 ± 5), DMA (64 ± 6), Roxarsone (18 ± 1), and four unidentified arsenic species (approximate concentration 1–10 μg kg⁻¹).     

Anionic cartridge preconcentrators for inorganic arsenic, monomethylarsonate and dimethylarsinate determination by on-line HPLC-HG-AAS

 Preconcentration anionic cartridges in combination with hyphenated FI-HG-AAS and HPLC-HG-AAS have been evaluated for the preconcentration and quantification of total toxic arsenic and of inorganic arsenic, monomethylarsonate and dimethylarsinate species, respectively. Optimum retention and elution parameters of the species on the anionic cartridges are evaluated and the quality parameters of the analysis are reported. The detection limits for the arsenic species under study range from 0.1 μg L^-1 to 0.6 μg L^-1. The proposed method was successfully applied to the determination of arsenic species in spiked fresh water. Received: 2 April 1996/Revised: 22 July 1996/Accepted: 25 July 1996     

Determination of arsenic(III) and total inorganic arsenic in water samples using an on-line sequential insertion system and hydride generation atomic absorption spectrometry

A simple and robust on-line sequential insertion system coupled with hydride generation atomic absorption spectrometry (HG-AAS) was developed, for selective As(III) and total inorganic arsenic determination without pre-reduction step. The proposed manifold, which is employing an integrated reaction chamber/gas-liquid separator (RC-GLS), is characterized by the ability of the successful managing of variable sample volumes (up to 25 ml), in order to achieve high sensitivity. Arsine is able to be selectively generated either from inorganic As(III) or from total arsenic, using different concentrations of HCl and NaBH₄ solutions. For 8 ml sample volume consumption, the sampling frequency is 40 h⁻¹. The detection limit is c_L = 0.1 and 0.06 μg l⁻¹ for As(III) and total arsenic, respectively. The precision (relative standard deviation) at 2.0 μg l⁻¹ (n = 10) level is s_r = 2.9 and 3.1% for As(III) and total arsenic, respectively. The performance of the proposed method was evaluated by analyzing the certified reference material NIST CRM 1643d and spiked water samples with various concentration ratios of As(III) to As(V). The method was applied for arsenic speciation in natural waters samples.     

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.     

Filtration through nylon membranes negatively affects analysis of arsenic and phosphate by the molybdenum blue method

Filtering synthetic arsenic- or phosphate-containing solutions (1.5-47.6 μmol/L) with nylon syringe filters significantly reduced absorbances (by 6-74%) when analyzed with the colorimetric molybdenum blue method. Filtering the same solutions with cellulose acetate syringe filters yielded no significant differences as compared to unfiltered controls. The detrimental effect of nylon membranes was also observed when pure Milli-Q water was filtered and subsequently spiked with arsenic(III) or phosphate suggesting that some compound(s) eluting from the filter membranes interfere with the color formation in the assay. Consequently, we caution against using nylon filters when filtering water samples for the determination of arsenic or phosphate with the molybdenum blue method.