Determination of 'arsenosugars' in algae with anion-exchange chromatography and an inductively coupled plasma mass spectrometer as element-specific detector

The retention behavior of four naturally occurring dimethylarsinoylribosides with -CH2-CHOH-CH2X (X = OH, HO3POCH2CHOHCH2OH, SO3H, OSO3H) as aglycones, of arsenous acid, arsenic acid, methylarsonic acid, and dimethylarsinic acid was investigated on a Hamilton PRP-X100 anion-exchange column with aqueous solutions of ammonium dihydrogen phosphate (20 mmol/L) in the pH range of 3.8-9.0 as mobile phase. A HP 4500 inductively coupled plasma mass spectrometer (ICP-MS) served as arsenic-specific detector. The influence of pH, temperature, and the concentration of methanol in the mobile phase on the retention times of these arsenic compounds was explored. An aqueous 20 mM ammonium dihydrogen phosphate solution at pH 5.6 at a column temperature of 40 degrees C was considered optimal as it allowed the separation of seven of the arsenic compounds within 16 min. Only arsenous acid and the ribose with the glycerol aglycone have overlapping signals with both migrating almost with the solvent front. At a concentration of 0.50 ng As mL(-1) the relative standard deviations (n = 3) of the signal areas of the eight arsenic compounds was in the range from 3.5 to 8.1%. The linear calibration curves (peak areas) from 0.5 to 10 ng/mL had correlation coefficients > 0.997. Extracts obtained from the brown algae Fucus spiralis and Halidrys siliquosa were chromatographed under the optimized conditions. Both species contained the sulfate riboside as the major arsenic compound (approximately 55% of total extractable arsenic) together with the sulfonate- and phosphate riboside. Arsenic acid was a significant constituent of Halidrys siliquosa (approximately 6.5%), but was not detected in Fucus spiralis.     

Speciation of arsenic compounds by coupling high-performance liquid chromatography with inductively coupled plasma mass spectrometry

There is considerable evidence that toxicity and physiological behavior of arsenic depends on its chemical forms. Arsenic speciation became therefore the subject of increasing interest in recent years. A sensitive method for the determination of arsenic species has been developed. The proposed procedure involves the use of high-performance liquid chromatography and inductively coupled plasma mass spectrometry (HPLC-ICP-MS). Six arsenic compounds were separated by anion-exchange chromatography with isocratic elution using tartaric acid as mobile phase with an elution order: arsenocholine, arsenobetaine, dimethylarsinic acid, methylarsonic acid, arsenous acid and arsenic acid. The chromatographic parameters affecting the separation of the arsenic species were optimized. Analytical characterization of the method has been realized with standard solutions. The detection limits for six arsenic compounds were from 0.04 to 0.6 g/L as As element. The repeatability (expressed by R.S.D) was better than 7% for all investigated compounds. The HPLC-ICP-MS system was successfully applied to the determination of arsenic compounds in environmental and biological samples in g/L level.     

Determination of bromide, bromate and other anions with ion chromatography and an inductively coupled plasma mass spectrometer as element-specific detector

An implementation of the Dionex IonPac AS12A analytical column with an element-specific ICP-MS detection is described for the simultaneous determination of halogen and oxyhalogen anions, sulfate, phosphate, selenite, selenate and arsenate. The chromatographic separation was achieved in less than 4 min with an aqueous 11 mM (NH4)2CO3 (pH 11.2, adjusted with aqueous ammonia) as eluent. Special emphasis was given to optimize the ICP-MS detection conditions for the reliable detection (RSD<5%) of bromate and bromide at a bromine concentration level of 1.0 microg l(-1) with 50 microl sample injection volume. In order to achieve the highest detector response for bromine species an ultrasonic nebulizer equipped with a membrane desolvator had to be employed. The detection limits (S/N=3, sample injection volume 50 microl) obtained with the IC-ICP-MS after the optimization were 0.67 microg l(-1) for BrO3-, 0.47 microg l(-1) for Br-, 69 microg l(-1) for ClO2-, 4 microg l(-1) for Cl-, 47 microg l(-1) for ClO3-, 13 microg l(-1) for SO4(2-), 36 microg l(-1) for PO4(3-), 0.4 microg l(-1) for SeO3(2-), 0.3 microg l(-1) for SeO4(2-), and 0.4 microg l(-1) for AsO4(3-).     

高效液相色谱-电感耦合等离子体质谱联用测定海洋产品中无机砷

采用高效液相色谱( HPLC)和电感耦合等离子体质谱(ICP-MS)联用技术测定了海洋产品中的无机砷.动物性和植物性海洋产品试样经过10％ H3PO溶液(V/V)提取,阴离子交换色谱分离,ICP-MS测定其中As(Ⅲ)和As(Ⅴ)的含量.实验结果表明As(Ⅲ)和As(Ⅴ)的检出限分别为5.0和8.0 μg/kg,线性范...     

Arsenic compounds in terrestrial organisms. IV. Green plants and lichens from an old arsenic smelter site in Austria

Two lichens and 12 green plants growing at a former arsenic roasting facility in Austria were analyzed for total arsenic by ICP–MS, and for 12 arsenic compounds (arsenous acid, arsenic acid, dimethylarsinic acid, methylarsonic acid, arsenobetaine, arsenocholine, trimethylarsine oxide, the tetramethylarsonium cation and four arsenoriboses) by HPLC–ICP–MS. Total arsenic concentrations were in the range of 0.27 mg As (kg dry mass)⁻¹ (Vaccinium vitis idaea) to 8.45 mg As (kg dry mass)⁻¹ (Equisetum pratense). Arsenic compounds were extracted with two different extractants [water or methanol/water (9:1)]. Extraction yields achieved with water [7% (Alectoria ochroleuca) to 71% (Equisetum pratense)] were higher than those with methanol/water (9:1) [4% (Alectoria ochroleuca) to 22% (Deschampsia cespitosa)]. The differences were caused mainly by better extraction of inorganic arsenic (green plants) and an arsenoribose (lichens) by water. Inorganic arsenic was detected in all extracts. Dimethylarsinic acid was identified in nine green plants. One of the lichens (Alectoria ochroleuca) contained traces of methylarsonic acid, and this compound was also detected in nine of the green plants. Arsenobetaine was a major arsenic compound in extracts of the lichens, but except for traces in the grass Deschampsia cespitosa, it was not detected in the green plants. In contrast to arsenobetaine, trimethylarsine oxide was found in all samples. The tetramethylarsonium cation was identified in the lichen Alectoria ochroleuca and in four green plants. With the exception of the needles of the tree Larix decidua the arsenoribose (2′R)‐dimethyl[1‐O‐(2′,3′‐dihydroxypropyl)‐5‐deoxy‐β‐D ‐ribofuranos‐5‐yl]arsine oxide was identified at the low μg kg⁻¹ level or as a trace in all plants investigated. In the lichens an unknown arsenic compound, which did not match any of the standard compounds available, was also detected. Arsenocholine and three of the arsenoriboses were not detected in the samples. Copyright © 2000 John Wiley & Sons, Ltd.     

Speciation of selenium compounds with ion-pair reversed-phase liquid chromatography using inductively coupled plasma mass spectrometry as element-specific detection

For selenium speciation analysis, the hyphenation of chromatographic separation with element-specific detection has proved a useful technique. A powerful separation system, which is capable of resolving several biologically and environmentally important selenium compounds in a single column, is greatly needed. However, that has been difficult to achieve. In this paper eight selenium compounds, namely, selenite [Se(IV)], selenate [Se(VI)], selenocystine (SeCys), selenourea (SeUr), selenomethionine (SeMet), selenoethionine (SeEt), selenocystamine (SeCM) and trimethylselenonium ion (TMSe+), were separated by using mixed ion-pair reagents containing 2.5 mM sodium 1-butanesulfonate and 8 mM tetramethylammonium hydroxide as a mobile phase. The separation of these anionic, cationic and neutral organic selenium compounds on a LiChrosorb RP18 reversed-phase column took only 18 min at a flow-rate of 1.0 ml/min with isocratic elution, and baseline separation among the six organic Se compounds was achieved. Inductively coupled plasma mass spectrometry (ICP-MS) was employed as element-specific detection. A comparison of ICP-MS signal intensity obtained with a Barbington-type nebulizer and with an ultrasonic nebulizer (USN) was made. Different signal enhancement factors were observed for the various selenium compounds when a USN was used. The speciation technique was successfully applied to the study on chemical forms of selenium in a selenium nutritional supplement. Selenomethionine was found to be the predominant constituent of selenium in the supplement.     

Determination of arsenic species by inductively coupled plasma mass spectrometry with ion chromatography

Five arsenic species, trimethylarsine oxide, dimethylarsenic acid, monomethylarsonic acid, arsenobetaine and sodium arsenite, in urine were analysed by inductively coupled plasma mass spectrometry with ion chromatography (IC ICP MS). Since the toxicities of different arsenic compounds are different, speciation of arsenic compounds is very important in the investigation of metabolisms. In this paper, we applied ion chromatography (IC) as a separation device and inductively coupled plasma mass spectrometry (ICP MS) as a detection device. For separation of the five arsenic compounds, an anion-exchange column and, as mobile phase, tartaric acid were used. The eluent from the IC column was introduced directly into the nebulizer of the ICP MS and analysed at 75 amu. Detection limits were from 4 to 9 pg as arsenic.     

Bromate assay in water by inductively coupled plasma mass spectrometry combined with solid-phase extraction cartridges

Based on selective sorption of bromide, bromoacetic acids (BAA) and bromomethanes on solid-phase extraction (SPE) cartridges, a sensitive and convenient method was developed for the determination of bromate in waters by inductively coupled plasma mass spectrometry (ICP–MS). Dionex OnGuard Ag and reversed-phase (RP) cartridges were tested for retention characteristics for bromide, BAA and bromomethanes. When a sample acidified with nitric acid was passed through an RP cartridge, BAA and bromomethanes were retained, afterwards bromide was absorbed as a precipitate of silver bromide and bromate was unretained when the nearly neutral sample passed a combination of Ag and H cartridges. After SPE pretreatment the recovery of bromate was 96–106%, and bromide remaining in the aqueous phase was found to be less than 0.06 g L^–1 when the original bromide concentrations were less than 5 mg L^–1. Effectiveness of stacked Ag and H cartridges in removing bromide from chloride-containing samples was also examined. Common cations and other anions did not interfere with bromate determination. The detection limit for bromate is 57 ng L^–1. This method has been applied to analyse waters from various sources, and the recovery of the spiked bromate was in the range of 92–107%.     

Determination of inorganic arsenic and organic arsenic compounds in marine organisms by hydride generation/cold trap/gas chromatography— mass spectrometry

The behavior of arsenite, methylarsonic acid, dimethylarsinic acid, trimethylarsine oxide, dimethyl-R-arsine oxides, and trimethyl-R-arsonium compounds (R = carboxymethyl, 2-carboxyethyl, 2-hydroxyethyl) toward sodium borohydride and hot aqueous sodium hydroxide was investigated. The arsines obtained by sodium borohydride reduction of the undigested and digested solutions were collected in a liquid-nitrogen cooled trap, separated with a gas chromatograph, and detected with a mass spectrometer in the selected-ion-monitoring mode. The investigated arsenic compounds were stable in hot 2 mol dm^?3 sodium hydroxide except arsenobetaine [trimethyl(carboxymethyl)arsonium zwitterion] that was converted to trimethylarsine oxide, and dimethyl(ribosyl)arsine oxides that were decomposed to dimethylarsinic acid. Hydride generation before and after digestion of extracts from marine organisms allowed inorganic arsenic, methylated arsenic, arsenobetaine, and ribosyl arsenic compounds to be identified and quantified. This method was applied to extracts from shellfish, fish, crustaceans, and seaweeds.     

Ion chromatography–inductively coupled plasma mass spectrometry determination of arsenic species in marine samples

Arsenic speciation analysis in marine samples was performed using ion chromatography (IC) with inductively coupled plasma mass spectrometry (ICP‐MS) detection. The separation of eight arsenic species, viz. arsenite, monomethyl arsonic acid, dimethylarsinic acid, arsenate, arsenobetaine, tetramethylarsine oxide, arsenocholine and tetramethylarsonium ion was achieved on a Dionex AS4A (weaker anion exchange column) by using a nitric acid pH gradient eluent (pH 3.3 to 1.3). The entire separation was accomplished in 12 min. The detection limits for the eight arsenic species by IC–ICP‐MS were in the range 0.03–1.6 µ g l^?1, based on 3σ of the blank response (n = 6). The repeatability and day‐to‐day reproducibility were calculated to be less than 10% (residual standard deviation) for all eight species. The method was validated by analyzing a certified reference material (DORM‐2, dogfish muscle) and then successfully applied to several marine samples, e.g. oyster, fish muscle, shrimp and marine algae. The low power microwave digestion was employed for the extraction of arsenic from seafood products. Copyright © 2004 John Wiley & Sons, Ltd.     

Speciation and health risk considerations of arsenic in the edible mushroom Laccaria amethystina collected from contaminated and uncontaminated locations

Samples of the edible mushroom Laccaria amethystina, which is known to accumulate arsenic, were collected from two uncontaminated beech forests and an arsenic-contaminated one in Denmark. The total arsenic concentration was 23 and 77 μg As g⁻¹ (dry weight) in the two uncontaminated samples and 1420 μg As g⁻¹ in the contaminated sample. The arsenic species were liberated from the samples using focused microwave-assisted extraction, and were separated and detected by anion- and cation-exchange high-performance liquid chromatography with an inductively coupled plasma mass spectrometer as arsenic-selective detector. Dimethylarsinic acid accounted for 68–74%, methylarsonic acid for 0.3–2.9%, trimethylarsine oxide for 0.6–2.0% and arsenic acid for 0.1–6.1% of the total arsenic. The unextractable fraction of arsenic ranged between 15 and 32%. The results also showed that when growing in the highly arsenate-contaminated soil (500–800 μg As g⁻¹) the mushrooms or their associated bacteria were able to biosynthesize dimethylarsinic acid from arsinic acid in the soil. Furthermore, arsenobetaine and trimethylarsine oxide were detected for the first time in Laccaria amethystina. Additionally, unidentified arsenic species were detected in the mushroom. The finding of arsenobetaine and trimethylarsine oxide in low amounts in the mushrooms showed that synthesis of this arsenical in nature is not restricted to marine biota. In order to minimize the toxicological risk of arsenic to humans it is recommended not to consume Laccaria amethystina mushrooms collected from the highly contaminated soil, because of a genotoxic effect of dimethylarsinic acid observed at high doses in animal experiments. © 1998 John Wiley & Sons, Ltd. No Abstract.     

Simultaneous separation of 17 inorganic and organic arsenic compounds in marine biota by means of high-performance liquid chromatography/inductively coupled plasma mass spectrometry

A method using high-performance liquid chromatography/inductively coupled plasma mass spectrometry (HPLC/ICP-MS) has been developed to determine inorganic arsenic (arsenite, arsenate) along with organic arsenic compounds (monomethylarsonic acid, dimethylarsinic acid, arsenobetaine, arsenocholine, trimethylarsine oxide, tetramethylarsonium ion and several arsenosugars) in fish, mussel, oyster and marine algae samples. The species were extracted by means of a methanol/water mixture and a dispersion unit in 2 min, with extraction efficiencies ranging from 83 to 107% in the different organisms. Up to 17 different species were determined within 15 min on an anion-exchange column, using a nitric acid gradient and an ion-pairing reagent. As all species are shown in one chromatogram, a clear overview of arsenic distribution patterns in different marine organisms is given. Arsenobetaine is the major compound in marine animals whereas arsenosugars and arsenate are dominant in marine algae. The method was validated with CRM DORM-2 (dogfish muscle). Concentrations were within the certified limits and low detection limits of 8 ng g(-1) (arsenite) to 50 ng g(-1) (arsenate) were obtained.     

Application of a mixed-gas microwave induced plasma as an on-line element-specific detector in high-performance liquid chromatography

Summary The applicability of a microwave induced plasma (MIP) as an on-line element-specific detector in high-performance liquid chromatography (HPLC) was investigated. A mixed gas oxygen-argon MIP sustained in a modified discharge tube consisting of two concentric quartz tubes, was used as an atomic emission detector for different mercury compounds. After passing the UV-vis detection cell of the HPLC system the eluent is nebulized and reaches the plasma without prior desolvation. The plasma tolerates methanol-water mixtures up to a methanol content of 90%. Detection limits for organically bound Hg are in the nanogram range. The sensitivity depends, however, on molecular structures. The capability of the HPLC-MIP is illustrated by the separation of some mercury species as 2-mercapto-ethanol complexes and by investigations of immobile mercury compounds in highland peat bog soil.

---

Anwendung eines mikrowelleninduzierten Mischgas-Plasmas als on-line elementspezifischer Detektor in der HPLC

Zusammenfassung Ein mikrowelleninduziertes Plasma (MIP) wurde on-line als elementspezifischer Detektor für durch HPLC getrennte, organische Hg-Verbindungen eingesetzt. Das als atomspektroskopische Anregungsquelle verwendete Sauerstoff-Argon-Plasma erfordert ein modifiziertes Entladungsgefäß mit getrennter Zuführung der beiden Gase. Die Elutionslösung strömt durch einen UV-vis-Detektor, wird dann pneumatisch zerstäubt und mit dem Argonstrom direkt in das Plasma transportiert, das Methanol-Wasser-Gemische mit Methanol-Gehalten von bis zu 90% verträgt. Die Nachweisgrenzen für organisch gebundenes Quecksilber liegen im Nanogrammbereich, hängen jedoch von der Struktur der jeweiligen Verbindung ab. Mit Hilfe des beschriebenen HPLC-MIP-Systems wurden einige Hg-Spezies als 2-Mercapto-ethanol-Komplexe getrennt und detektiert, sowie Untersuchungen über immobile Hg-Verbindungen in Hochmoortorfböden durchgeführt.

---

---

Dedicated to Prof. Dr. K. Laqua on the occasion of his 65. birthday     

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.     

Distribution and fate of biologically formed organoarsenicals in coastal marine sediment

Marine organisms, including phyto‐ and zoo‐plankton, macroalgae, and animals, concentrate arsenic in various organic forms. However, the distribution and fate of these organoarsenicals in marine environments remains unclear. In this study, the distribution of organoarsenicals in coastal marine sediment in Otsuchi Bay, Japan, has been determined. Methylarsonic acid, dimethylarsinic acid, trimethylarsine oxide, arsenobetaine, arsenocholine and other unidentified arsenic species were detected in marine sediment by high‐performance liquid chromatography–inductively coupled plasma mass spectrometry analysis of methanol–water extracts. Arsenobetaine was the dominant organoarsenical at four of the seven stations where tests were carried out, and unidentified species or dimethylarsinic acid dominated at the other stations. Total organoarsenicals (as arsenic) in the surface sediment amounted to 10.6–47.5 µg kg^?1 dry sediment. Core analysis revealed that concentrations of organoarsenicals decreased with depth, and they are considered to be degraded within 60 years of deposition. These results show that organoarsenicals formed by marine organisms are delivered to the sediment and can be degraded within several decades. Copyright © 2005 John Wiley & Sons, Ltd.     

Determination of organometallic compounds by capillar gas chromatography – inductively coupled plasma mass spectrometry

The separation and detection of volatile organometallic compounds containing tin, iron, and nickel has been achieved using capillary GC–inductively coupled plasma–mass spectrometry (capillary GC-ICP-MS). Detection limits range from 3.0 to 7.0 pg/s. The presence of volatile organotin compounds in a harbor sediment has been confirmed. The retention range of the organometallic compounds analyzed by capillary GC-ICP-MS has been extended considerably beyond that possible in earlier studies (retention indices up to 3400).     

A study of the interactions between carboplatin and blood plasma proteins using size exclusion chromatography coupled to inductively coupled plasma mass spectrometry

To study the carboplatin–protein interaction, a sensitive method using size exclusion chromatography coupled to inductively coupled plasma mass spectrometry (SEC–ICP–MS) was developed. The complexes formed between plasma proteins and carboplatin were monitored and identified with this method. Composite blood plasma samples from patients who were undergoing chemotherapy were analyzed, and carboplatin was found to bind plasma proteins. In addition, blank plasma samples were spiked with carboplatin and were analyzed as a time course study, and the results confirmed that carboplatin formed complexes with plasma proteins, primarily albumin and γ-globulin. To further substantiate the study, these two proteins were incubated with carboplatin. The binding between carboplatin and these proteins was then characterized qualitatively and quantitatively. In addition to a one-to-one binding of Pt to protein, protein aggregation was observed. The kinetics of the binding process of carboplatin to albumin and γ-globulin was also studied. The initial reaction rate constant of carboplatin binding to albumin was determined to be 0.74 M⁻¹ min⁻¹, while that for γ-globulin was 1.01 M⁻¹ min⁻¹, which are both lower than the rate constant of the cisplatin–albumin reaction previously reported.     

An ultrafiltration high-performance liquid chromatography coupled with diode array detector and mass spectrometry approach for screening and characterising tyrosinase inhibitors from mulberry leaves

Tyrosinase is a key enzyme in melanin synthesis. Its inhibitor may be used to efficiently treat hyperpigmentation and widely applied in cosmetic products and food supplements. In the present study, a new assay based on ultrafiltration high-performance liquid chromatography coupled with diode array detector and mass spectrometry (HPLC–DAD–MS) was developed for the rapid screening and identification of ligands for tyrosinase. Experiments were carried out to select the optimal binding conditions, tyrosinase concentration, and incubation time. Non-specific binding to the denatured tyrosinase was also investigated. Twelve compounds with tyrosinase binding activity were found in mulberry leaf extracts. The identities of these compounds were characterised by HPLC–DAD–MSⁿ. Particularly, two compounds, namely, quercetin-3-O-(6-O-malonyl)-β-d-glucopyranoside and kaempferol-3-O-(6-O-malonyl)-β-d-glucopyranoside, were identified as new tyrosinase inhibitors. The screening results were verified by tyrosinase inhibition assays. Experimental results proved that the proposed method could rapidly screen tyrosinase inhibitors in complex mixtures.     

Organoarsenic compounds in plants and soil on top of an ore vein

Plants and soil collected above an ore vein in Gasen (Austria) were investigated for total arsenic concentrations by inductively coupled plasma mass spectrometry (ICP‐MS). Total arsenic concentrations in all samples were higher than those usually found at non‐contaminated sites. The arsenic concentration in the soil ranged from ∼700 to ∼4000 mg kg⁻¹ dry mass. Arsenic concentrations in plant samples ranged from ∼0.5 to 6 mg kg⁻¹ dry mass and varied with plant species and plant part. Examination of plant and soil extracts by high‐performance liquid chromatography–ICP‐MS revealed that only small amounts of arsenic (<1%) could be extracted from the soil and the main part of the extractable arsenic from soil was inorganic arsenic, dominated by arsenate. Trimethylarsine oxide and arsenobetaine were also detected as minor compounds in soil. The extracts of the plants (Trifolium pratense, Dactylis glomerata, and Plantago lanceolata) contained arsenate, arsenite, methylarsonic acid, dimethylarsinic acid, trimethylarsine oxide, the tetramethylarsonium ion, arsenobetaine, and arsenocholine (2.5–12% extraction efficiency). The arsenic compounds and their concentrations differed with plant species. The extracts of D. glomerata and P. lanceolata contained mainly inorganic arsenic compounds typical of most other plants. T. pratense, on the other hand, contained mainly organic arsenicals and the major compound was methylarsonic acid. Copyright © 2002 John Wiley & Sons, Ltd.     

Arsenic Compounds in Higher Fungi

In 50 mushroom species (56 samples) from Slovenia, Switzerland, Brazil, Sweden, The Netherlands and USA, total arsenic was determined by radiochemical neutron activation analysis (RNAA). Arsenic concentrations ranged from 0.1 to 30 μg g⁻¹ (dry mass). Arsenic compounds were determined in methanol extracts from the mushrooms by HPLC–ICP–MS. The aim of the study was not only to quantify arsenic compounds in mushrooms but also to uncover trends relating the methylating ability of a mushroom to its taxonomic or evolutionary status. The main arsenic compound found in many mushrooms (various puffballs, Agaricales and Aphyllophorales) was arsenobetaine. Arsenate [As(V)] was the main arsenic species in Laccaria fraterna and Entoloma rhodopolium and arsenite [As(III)] in Tricholoma sulphureum. A mixture of arsenite and arsenate was present in Amanita caesarea. Dimethylarsinic acid (DMA) and methylarsonic acid were present in many mushrooms, but generally as minor components. In Laccaria laccata, Leucocoprinus badhamii and Volvariella volvacea, DMA was the major metabolite. Arsenocholine (AC) and the tetramethylarsonium ion were present in a few species, generally at low concentrations, except for Sparassis crispa, in which AC was the main compound. Tri- methylarsine oxide was not found in any of the mushrooms. In some species small amounts of unknown compounds were also present. The possible taxonomic significance of the metabolite patterns and the predominance of arsenobetaine in more advanced fungal types are discussed. © 1997 John Wiley & Sons, Ltd.