Determination of Cd,Mo, Cr and Co in biological materials by RNAA

A method for the determination of trace amounts of Mo, Cd, Co and Cr in biological materials by neutron activation analysis with radiochemical separation is presented. The method is based on the ion-exchange scheme developed by SAMSAHL, where Co and Cr are trapped on BioRad Chelex-100 and Cd and Mo on BioRad AG2X8. The elements Mo, Cd and Co can be determined without systematic errors. For the element chromium the situation is less clear, partially due to lack of sufficient certified reference materials for Cr. The method has been used in the characterization of candidate reference materials. Detection limits in these materials range from 1.5 g/kg for Co to 10 g/kg for Cr. Actual levels as low as 8 g/kg for Cd and 7 g/kg for Co were measured.     

Determination of trace Cd and Pb in environmental and biological samples by ETV-ICP-MS after single-drop microextraction

A method based on single-drop microextraction (SDME) combined with electrothermal vaporization (ETV)-ICP-MS was proposed for the determination of trace Cd and Pb. 8-Hydroxyquinoline (8-HQ) was employed as extractant dissolved in several microliters of chloroform and then an organic microdrop was formed at the tip of the microsyringe needle to extract the interest analytes. The vaporization behavior of the metal-8-HQ chelates in graphite furnace was investigated, and the ETV temperature program was optimized. The factors that influenced the extraction efficiency of target analytes (including pH value, flow rate of sample, extraction time and organic microdrop volume) were studied. Under the optimum conditions, the detection limits of the Cd and Pb were 4.6 and 2.9 pg mL⁻¹ with the enrichment factor of 140-fold for Cd and 190-fold for Pb, respectively. The proposed method was applied successfully to the determination of trace Cd and Pb in environmental and biological samples. In order to validate the developed method, a certified reference material of GBW 08501 peach leaves was analyzed and the determined values obtained were in a good agreement with the certified values.     

Simultaneous determination of hydride forming elements (As, Sb, Se, Sn) and Hg in sonicate slurries of biological and environmental reference materials by hydride generation microwave induced plasma optical emission spectrometry (SS-HG-MIP-OES)

A slurry sampling hydride generation (SS-HG) method for the simultaneous determination of hydride forming elements (As, Sb, Se, Sn) and Hg, without total sample digestion, has been developed using batch mode generation system coupled with microwave induced plasma optical emission spectrometry (MIP-OES) from certified biological and environmental reference materials. Slurry concentration up to 3.6% m/v (particles < 80 μm) prepared in 10% HCl containing 100 μl of decanol, by the application of ultrasonic agitation, was used with calibration by the standard addition technique. Harsh conditions were used in the slurry preparation in order to reduce the hydride forming elements to their lower oxidation states, As(III), Sb(III), Se(IV) and Sn(II) and Hg, being reduced to mercury vapor, before reacting with sodium tetrahydroborate. An ultrasonic probe was used to homogenize the slurry in the quartz cup just before its introduction into the reaction vessel. For 10 ml of slurry sample, detection limits (LOD, 3σ_blank, peak area) of 0.06, 0.08, 0.15, 0.12 and 0.10 μg g^− 1 were obtained for As, Sb, Se, Sn and Hg, respectively. The method offers relatively good precision (RSD ranged from 9 to 12%) for slurry analysis. To test the accuracy, three certified reference materials were analyzed with the analyte concentrations mostly in the μg g^− 1 level. Measured concentrations are in satisfactory agreement with certified values for the biological reference materials: NRCC LUTS-1 (lobster hepatopancreas), NRCC DOLT-2 (Dogfish Liver) and environmental reference material: NRCC PACS-1 (Marine Sediment), all adequate for slurry sampling. The method requires small amounts of reagents and reduces contamination and losses.     

Lead determination in slurries of biological materials by ETAAS using a W-Rh permanent modifier

A tungsten-rhodium coating on the integrated platform of a transversely heated graphite atomiser (THGA) was used as a permanent chemical modifier for the determination of lead in biological materials by slurry sampling in electrothermal atomic absorption spectrometry (ETAAS). Slurries were sonicated during 20 s before being delivered to the previously W-Rh treated platform. The number of particles of biological materials introduced into the atomiser for delivering 20 microL slurry aliquot ranged from 5,100 to 39,000. The permanent W-Rh modifier remained stable during approximately 300 analytical measurements when 20 microL of slurries containing up to 1.5% m/v were delivered into the atomiser. In addition, the permanent modifier increases the tube lifetime by approximately 100% when compared to untreated integrated platforms. Also, there is less decrease of sensitivity during the atomiser lifetime when compared with the conventional modifiers, resulting in a decreased need of re-calibration during routine analysis and consequently increasing the sample throughput. The atomiser lifetime was limited to the THGA wall durability, because the W-Rh treated platform was intact after more than 650 analytical firings in a medium containing up to 1.5% m/v slurry of biological material. The detection limit based on integrated absorbance was 20 ng g(-1) Pb for 1.50% m/v slurries. Results from the determination of lead in slurries of biological materials using the W-Rh permanent modifier were in agreement with those obtained with digested solutions using Pd + Mg(NO3)2.     

Lead determination in slurries of biological materials by ETAAS using a W-Rh permanent modifier

A tungsten-rhodium coating on the integrated platform of a transversely heated graphite atomiser (THGA) was used as a permanent chemical modifier for the determination of lead in biological materials by slurry sampling in electrothermal atomic absorption spectrometry (ETAAS). Slurries were sonicated during 20 s before being delivered to the previously W-Rh treated platform. The number of particles of biological materials introduced into the atomiser for delivering 20 μL slurry aliquot ranged from 5,100 to 39,000. The permanent W-Rh modifier remained stable during approximately 300 analytical measurements when 20 μL of slurries containing up to 1.5% m/v were delivered into the atomiser. In addition, the permanent modifier increases the tube lifetime by approximately 100% when compared to untreated integrated platforms. Also, there is less decrease of sensitivity during the atomiser lifetime when compared with the conventional modifiers, resulting in a decreased need of re-calibration during routine analysis and consequently increasing the sample throughput. The atomiser lifetime was limited to the THGA wall durability, because the W-Rh treated platform was intact after more than 650 analytical firings in a medium containing up to 1.5% m/v slurry of biological material. The detection limit based on integrated absorbance was 20 ng g^–1 Pb for 1.50% m/v slurries. Results from the determination of lead in slurries of biological materials using the W-Rh permanent modifier were in agreement with those obtained with digested solutions using Pd + Mg(NO₃)₂. Received: 11 August 2000 / Revised: 13 November 2000 / Accepted: 16 November 2000     

Determination of Cd and Pb in food slurries by GFAAS using cryogenic grinding for sample preparation

A simple method combining slurry sampling after cryogenic grinding and the use of a permanent modification of the integrated platform inside the transversely heated graphite atomizer (THGA) was proposed for the determination of Cd and Pb in foods. Potentialities of the cryogenic grinding were evaluated for grinding different materials of difficult homogenization such as high fat and high fiber tissues. Animal and vegetal samples were cut into small pieces and ground in liquid nitrogen for 2 min. Slurries were prepared directly in the autosampler cup after cryogenic grinding by transferring an exact amount of homogeneous powdered material (5-20 mg) to the cup, followed by 1.00 mL of 0.2% (v/v) HNO3 containing 0.04% (v/v) Triton X-100 and sonication for 30 s, before transferring into the platform previously coated with 250 microg W and 200 microg Rh. Use of a tungsten carbide-rhodium permanent modifier combined with NH4H2PO4 conventional modifier improves tube lifetime and increases the pyrolysis temperature for Cd. Homogeneity tests, carried out by comparing the between- and within-batch precision for each kind of sample, showed no significant differences at the 95% confidence level, indicating good homogeneity for 5-20 mg masses. Detection limits were 3.3 ng g(-1) Cd and 75 ng g(-1) Pb for 1% m/v slurries. Results for determination of Cd and Pb in foods slurries were in agreement with those obtained with digested samples, since no statistical differences were found by the paired t-test at the 95% level.     

同位素稀释电感耦合等离子体质谱测定环境和生物样品中的镉

应用同位素稀释电感耦合等离子体质谱（ID—ICP—MS）对环境和生物样品茶叶、湖沉积物和人发标准物质中的镉进行测定研究。对电感耦合等离子体质谱（ICP—MS）的工作条件和参数进行了最优化。讨论了多原子离子和同量异位素对镉同位素比值的影响,通过天然镉标准溶液对质量歧视进行了校正,并优化同位素稀释剂的加入量。将该方法应用于茶叶、人发和沉积物标准物质的测定。     

Analysis of plutonium in biological and environmental materials

A procedure for separation of plutonium from some biological and environmental materials has been tested in model and real conditions. The procedure involves a commonly used way of conversion of plutonium to oxidation state (IV) in nitric acid medium and sorption of Pu(IV) on a strongly basic anion exchanger from hydrochloric acid medium thus eliminating interference of²²⁸Th with the²³⁸Pu analysis.     

Determination of bromine and iodine in biological and environmental materials using epithermal neutron activation analysis

Epithermal neutron activation analysis (ENAA) was applied to the determination of the contents of bromine and iodine in 40 biological and environmental standard reference materials and Chinese diets. Boron nitride (BN) for solid samples and BN+Cd for liquid samples were adopted as shield material. Irradiation was carried out in inner and outer irradiation sites in a Miniature Source Reactor (MNSR) for solid and liquid samples, respectively. The 443 keV photopeak of ¹²⁸I and the 616 keV photopeak of ⁸⁰Br were used. The precision of measurement (relative standard deviation) is 2∼6% for contents of iodine of more than 100 ng/g and 8∼12% in the 20∼100 ng/g range in solid samples, and 12∼18% at less than 100 ng/ml in liquid samples. For bromine, the precision of measurement is 2–8% for solid samples and lower than 13% for liquid samples. The detection limits under experimental conditions varied between 10∼30 ng/g, 55∼95 ng/g and 25∼68 ng/g for iodine and 50∼150 ng/g, 200∼450 ng/g and 100∼300 ng/g for bromine in ENAA with BN shield in inner irradiation sites, with Cd shield and BN+Cd shield in outer irradiation sites, respectively. Received: 13 June 1996 / Revised: 2 September 1996 / Accepted: 19 September 1996     

Elements very rapidly measurable by INAA in biological and environmental materials

In connection with the increasing usage of reference materials in INAA work, and with the continuing interest in this laboratory in rapid analyses via very short-lived induced activities, 13 biological and 8 environmental reference materials have been processed, under rapid analysis conditions, by the reactor-flux INAA Advance Prediction Computer Program. The results described show that a total of 33 induced (n, ) activities of 26 elements are detectable in these 21 reference materials, in total analysis times ranging from 1.5 to 192 seconds.     

Determination of cadmium in biological materials by atomic absorption

A variety of biological samples such as blood, urine, hair, nail and kidneys has been analysed cadmium. Tantalum ribbon flameless and conventional flame-aspiration atomic-absorption techniques were employed for the analysis.     

Determination of molybdenum in biological materials by neutron activation

A method of the determination of molybdenum in biological materials by neutron activation is described. The method is based on the γ-spectrometric measurement of^99mTc after radiochemical separation of the latter by substoichiometric extraction with tetraphenylarsonium chloride using rhenium as inactive carrier. The method has been tested with reference materials.     

Direct mercury determination in aqueous slurries of environmental and biological samples by cold vapour generation-electrothermal atomic absorption spectrometry

Direct cold vapour generation from aqueous slurries of environmental (marine sediment, soil, coal) and biological (human hair, seafood) samples have been developed using a batch mode generation system coupled with electrothermal atomic absorption spectroscopy. The effects of several variables affecting the cold vapour generation efficiency from solid particles (hydrochloric acid and sodium tetrahydroborate concentrations, argon flow rate, acid solution volume and mean particle size) have been evaluated using a Plackett-Burman experimental design. In addition, variables affecting cold vapour trapping and atomisation efficiency on Ir-treated graphite tubes (trapping and atomisation temperatures and trapping time) have been also investigated. Atomisation and trapping temperatures, trapping time and hydrochloric acid concentration were the significant variables. The 2²+star and 2³+star central composite designs have been used to obtain optimum values of the variables selected. The accuracy of methods have been verified by using several certified reference materials (PACS-1, GBW-07410, NIST-1632c, CRM-397 and DORM-2). A characteristic mass of 390 pg were achieved. The detection limits of methods were in the range of 40-600 ng g⁻¹. A particle size less than 50 μm is adequate to obtain total cold vapour generation of Hg content in the aqueous slurry particles.     

Pretreatment studies with biological and environmental materials

Summary A complete and down to the ultratrace level, i.e. down to a few ng/kg, nearly contamination free digestion for the subsequent mercury determination is possible in quartz vessels with HNO₃/HClO₄ mixtures (heating block, temperature up to 200°C). Very low mercury contents require especially purified acids. Vessels with volumes from 10 to 250 ml permit the digestion of samples up to 4g dry weight and 10g fresh weight. Duration of digestion depends on the matrix. For body fluids, tissue and plant materials typically approx. 1.5 h are required, for fatty materials 3 h and for sewage sludge approx. 8 h. A complete digestion of fatty materials is only possible in closed vessels with slight overpressure.

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Probenvorbehandlungsstudien mit biologischen und UmweltmaterialienIV. Vollständiger Naßaufschluß in teilweise und vollständig geschlossenen Quarzgefäßen zur nachfolgenden Spuren- und Ultraspurenbestimmung von Quecksilber

Zusammenfassung Ein vollständiger und bis in den Ultraspurenbereich, d.h. bis zu wenigen ng/kg, nahezu kontaminationsfreier Aufschluß zur Quecksilberbestimmung ist mit HNO₃/HClO₄-Gemischen in Quarzgefäßen (Heizblocktemperatur bis 200°C) möglich. Für sehr niedrige Gehalte müssen die verwendeten Säuren nachgereinigt werden. In Gefäßen von 10 bis 250 ml Inhalt können Probenmengen bis 4g Trocken- und 10 g Frischgewicht aufgeschlossen werden. Die Auf Schlußzeiten sind von der jeweiligen Probenmatrix abhängig und betragen für Körperflüssigkeiten, Gewebe- und Pflanzenmaterial etwa 1,5 h, für fetthaltiges Material etwa 3 h, für Klärschlamm etwa 8 h. Ein vollständiger Aufschluß fetthaltigen Materials ist nur im geschlossenen System mit leichtem Überdruck möglich.

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Dedicated to Prof. Dr. W. Fresenius on the occasion of his 70th birthday     

Pretreatment studies with biological and environmental materials

Summary In various biological and environmental materials the pressure pattern in closed teflon crucibles was followed after addition of nitric acid and heating. Hereby a significant influence of the matrix, of the temperature program and of the acid amount added on the pressure pattern was observed. The carbon balance, determined with the aid of gas-chromatography in several selected materials showed in no case a complete ashing and a very strong dependence of the decomposition rate on the kind of the investigated material.Part I: Fresenius Z. Anal. Chem. 291, 116 (1978); Part II: Fresenius Z. Anal. Chem. 293, 127 (1978)     

Pretreatment studies with biological and environmental materials

Summary Pressure digestion units made from stainless steel, with up to 12 sample positions, are described. The sizes of the teflon digestion crucibles are 0.6 resp. 35 ml for sample weights (dry weights) from about 10 up to 1000 mg. The handling of the units and the digestion crucibles, the standard digestion program with nitric acid (needed time including cooling period about 3 h), its evaluation and the very important safety aspects are extensively discussed.Supported by research grant MT 405 g/AUT 03 from the German Federal Department of Research and Technology (BMFT), Bonn, FRG