Arsenic speciation in Portuguese in situ lichen samples.

In this work, 29 lichen samples collected in situ and representative of high loadings, medium loadings and zero loadings for factors related to natural and anthropogenic emission sources, were analyzed to determine arsenic contents and its species extractability. The studied sites showed As values between 430 and 5590 microg kg(-1). The cationic forms were extracted at most of the sites varying between 0.5% and 6.6%. Extracted anionic forms were not detected in any of the sites. In a few other sites the % of extracted As(III)--more toxic--exceeds the equivalent value of As(V). It is concluded that arsenic in native Parmelia sulcata Taylor under the form of As(V) either was kept unchanged or was partially transformed into As(III) (more frequent) or partially transformed into As(III) and dimethylarsinic acid (DMAA) or partially transformed into DMAA.

Topical isotopic exchange and compartmental analysis approach for probing solute behaviour at the soil/arsenate solution interface.

Isotopic exchange based approaches have for many years been applied in soil and solute research. However, acquiring and elaboration of experimental data were not always straightforward and complete. A strict and correct use of combined isotopic exchange-compartmental analysis may widen the knowledge database and provide information not available as yet. The experiments were carried out with arsenic (arsenate) from IAEA-SOIL-5 in contact with water or phosphate solution in dynamic equilibrium. After contacting the soil suspension for 28 days, the amount of arsenate released is 2.8 and 6.3 % of arsenic (solutes) in the soil, respectively. Addition of a radioactive arsenate (73)As(V)-spike and following the distribution of this radiotracer from the aqueous to the solid phase in time shows that the accessible fraction, i.e. available for exchange, is in both cases 12%. This implies that the remainder of the arsenic is enclosed in the lattice of minerals and for that reason unavailable for exchange, at least on the time scale of the experiment (weeks). From deconvolution of compartmental analysis results the distribution of accessible arsenate in the soil could be attributed to sorption onto external surfaces (2.6 and 2.0% of total arsenic present for the water and phosphate system, respectively) and sorption onto internal surfaces after diffusion through soil particle pores (6.5 and 4.2% of total arsenic present for the water and phosphate system, respectively). The mean residence time in two out of three compartments was in the order of minutes for the external surfaces and in the order of days for the diffusion-controlled internal surfaces.

Determination of ultratrace dissolved arsenite in water--selective coprecipitation in the field combined with HGAFS and ICP-MS measurement in the laboratory.

Because stabilization of arsenite in water samples during transit and storage is troublesome, this work deals with a method to prevent this by on-site selective coprecipitation of arsenite with dibenzyldithiocarbamate and recovery of the coprecipitate by filtration through a 0.45-microm membrane filter. In the laboratory arsenic on the filter is quantitatively released by oxidation of arsenite to arsenate with H2O2 (6%) in alkaline medium (8 mmol L(-1) NaOH) at elevated temperature (85 degrees C) for 30 min followed by ultratrace determination by routine HGAFS and ICP-MS. It is shown that arsenate contamination of the coprecipitate is so low that arsenate concentrations three orders of magnitude higher than the arsenite concentration do not interfere; this is essential, because arsenate is usually the dominant arsenic species in water. Because significant preconcentration can be achieved in the solution obtained from the leached filter (normally a factor 20 but easily increased to 100) very low detection limits can be obtained (only limited by the purity of the materials and the cleanliness of working); a realistic limit of determination is 0.01 microg L(-1) arsenite. The procedure was used for the determination of arsenite in two ground waters from an ash depository site in the Salek valley (Slovenia). The matrix contained some elements at very high levels but this did not impair the efficiency of arsenite coprecipitation. The results obtained by use of HGAFS and ICP-MS were not significantly different at the 5% level for sub-microg L(-1) arsenite concentrations.

Preliminary study on the determination of selenium compounds in some selenium-accumulating mushrooms.

Using various chromatographic techniques (size exclusion, anion exchange, and cation exchange) combined with several detectors (neutron activation analysis and atomic fluorescence spectrometry), an attempt was made to characterize selenium compounds in some edible, selenium-accumulating mushrooms (Albatrellus pes-caprae and Boletus edulis). The mushrooms contained mostly low-molecular-weight (6 kDa) selenium compounds. After proteolysis, only a small fraction of the extractable selenium could be identified as selenite (3.0-9.2%, Albatrellus pes-caprae), selenocystine (minor, Albatrellus pes-caprae; 7.5%, Boletus edulis), or selenomethionine (1.0%, Boletus edulis), leaving the form of the bulk still to be elucidated.

Speciation of arsenic in coarse and fine urban aerosols using sequential extraction combined with liquid chromatography and atomic fluorescence detection.

An analytical procedure for speciation of As in urban aerosol samples was developed. The aerosols were collected by sequential filtration through membrane filters. Part of each filter was investigated by INAA for the total amount of As. Another part of the filters was treated by a sequential extraction procedure to differentiate between water-extractable, phosphate-extractable and refractory chemical forms. Water-extractable forms were further differentiated into anionic As species by HPLC-HGAFS. Extractability of As into water exhibited a clear dependency on the aerosol size fraction (12% in coarse fraction and 50% in fine fraction). Dependency of the phosphate extractable As on the aerosol size fraction seems not to be significant (10-15% in both size fractions). The remaining amount, i.e., about 78% of the coarse As and about 40% of the fine As was considered to be refractory or environmentally immobile As. Water-extractable As forms could only be attributed to arsenate.

Effect of arsenic trioxide on metallothionein and its conversion to different arsenic metabolites in hen liver.

The metabolism of arsenic, its affinity to metallothionein (MT), its influence on selenium levels, and its biotransformation to different metabolites in the liver tissue of laying hens exposed to arsenic trioxide (As2O3) was investigated. The experiment was performed with two groups of hens fed for 19 d with either a standard diet or with the same diet enriched in arsenic (30 microg/g). The major findings were as follows: 1. After 19 d exposure, about 65% of the total liver As was found in the water-soluble phase (100,000g centrifuged supernatant). In liver supernatant, As binding was found mostly in the range of very low-molecular-weight proteins (Mr < 10,000). Although after exposure the amount of MT-like proteins increased, the As bound to it was only in trace amounts. The protein was identified by convential procedures as Zn,Cu-thionein with traces of selenium and arsenic. 2. Arsenic exposure resulted in almost unchanged Se levels regarding its tissue concentrations and distribution between supernatant and pellet, where about 10% of total Se was found in the supernatant. On the contrary, As exposure did affect Cd levels. Tissue Cd concentration was slightly diminished, but the percentage of tissue Cd found in the water-soluble phase was increased from 20% to 40%. 3. In methanol extracts of tissue and supernatant of the As-exposed group, only two arsenic compounds were detected, As(III) and dimethylarsinic acid (DMA), the latter prevailing.

Understanding of peak deterioration in hyphenated speciation systems due to gas-liquid separation in the hydride generation interface.

In hyphenated speciation systems with a hydride generation interface one of the processes influencing peak deterioration is gas-liquid separation. A mathematical model was developed to calculate attenuation, signal tailing and resolution loss of HPLC peaks due to gas-liquid separation. It was shown experimentally--using an HPLC-hydride generation-atomic fluorescence spectrometry system for arsenic speciation--that the mathematical model predicts peak deterioration well. This allowed us to study the parameters influencing the deterioration, viz. gas-liquid separation parameters (gas-liquid separator head space volume and purge gas volume flow-rate) and HPLC peak parameters [width (ratio) and resolution] theoretically, simulating HPLC peaks with gaussian functions.

Determination of arsenic compounds in reference materials by HPLC-(UV)-HG-AFS.

Arsenic compounds were determined in six reference materials of biological origin. None of them has yet been certified for arsenic compounds but some are in the process of certification; for most of these reference materials indicative literature values are available. Eight commonly used arsenic standards were used for quantification using a recently developed hyphenated speciation system comprising high performance liquid chromatography (HPLC) and atomic fluorescence spectrometry (AFS), interfaced via a UV-photoreactor and a hydride generation (HG) unit. Absolute detection limits were ca. 0.2 and 0.4 ng As for separation on anion and cation exchange columns, respectively. Our results agree well with indicative literature values which were generated by different authors using various separation and detection methods. The HPLC-(UV)-HG-AFS system validated in this way is suitable for quantification of eight arsenic compounds. Moreover, the system is capable of separation of at least six more compounds in the mentioned reference materials, of which two could be attributed to arsenosugars (OH and phosphodiester form) but due to the lack of standards, quantification was not possible. For accurate and extensive speciation analysis the availability of certified reference materials and standards for arsenic compounds should be promoted.

Ion-exchange separation of eight arsenic compounds by high-performance liquid chromatography-UV decomposition-hydride generation-atomic fluorescence spectrometry and stability tests for food treatment procedures.

A novel separation for cationic arsenic compounds on a polymer-based cation-exchange column was developed using an ion-pairing reagent (3-carboxy-4-hydroxybenzenesulphonic acid) in the mobile phase. An existing anion-exchange separation was used for anionic arsenic compounds. Combining both separation techniques, eight environmentally important arsenic compounds can be determined using on-line decomposition in a UV reactor prior to hydride generation (HG) and atomic fluorescence spectrometry (AFS). The method was applied for testing the stability of arsenic compounds (in aqueous media) related to food treatment procedures. Boiling and microwave treatment gave no degradation, whereas gamma-irradiation and dry heating resulted in partial decomposition of several arsenic compounds. No health hazards are to be expected when these data are extrapolated to commercial or domestic food treatment procedures.

Applicability of neutron activation analysis (NAA) in quantitative determination of some essential and toxic trace elements in food articles.

Accurate and reliable data on microgram and nanogram quantities of some essential and toxic elements in most food articles are very scarce. Neutron activation analysis (NAA), with its essentially blankfree advantage, is a valuable approach in the field of determination of trace elements in different foodstuffs and diets. Accordingly, various radiochemical (RNAA) and instrumental (INAA) approaches have been developed in our laboratory for the element As, Cd, Co, Cu, Hg, I, Mo, Ni, Sb, Se, Sn, Th, U, V, and others, and verified by the analysis of compositionally appropriate certified reference materials.

Preliminary studies on arsenic species in some environmental samples.

Arsenic compounds have been determined in some environmental samples from the German Environmental Specimen Bank (ESB) (marine mussels, freshwater mussel and fish, sea-gull eggs) and certified reference materials (DORM-1, DOLT-1, NBS Oyster Tissue) after separation by open column cation and anion exchange chromatography by two different methods of total arsenic determination in separated fractions (instrumental neutron activation analysis or hydride generation atomic absorption spectrometry). Arsenobetaine has been identified as the major species in all the different materials.

Rapid radiochemical neutron activation analysis for iodine in urine by different separation techniques.

In the present work on radiochemical neutron activation analysis for the determination of iodine in urine samples, the performance of three different radiochemical separation techniques, namely, direct extraction, use of an iodinated ion-exchange resin column and Schöniger combustion, were intercompared and validated. The practical advantages of the iodinated-resin technique make it most suitable for the rapid routine determination of iodine in urine. It was further verified by participation in an international intercomparison run of urine analysis, and used in a pilot study on iodine determination in the urine of 171 Slovenian schoolchildren, where it gave results in good agreement with the catalytic method.