Direct determination of selenium in sub-milligram amounts of human sperm nuclei by electrothermal atomic absorption spectrometry

In the sperm nuclei selenium is present only in form of a single selenoenzyme, the sperm nuclei glutathione peroxidase (snGPx), involved in processes to secure the structural stability of the nuclear chromatin. As changes in its expression may affect sperm function, its analysis is of interest in the diagnosis of male infertility. A method has been developed which by removal of the other selenium compounds present in other sperm components and measurement of the concentration of selenium in the purified human sperm nuclei by electrothermal atomic absorption spectrometry (ETAAS) allows the quantitative analysis of this enzyme. As the purification resulted in yields in the range of only 150 μg nuclei/ml semen and the amount of purified nuclei in the sample could only be determined by weighing, the main analytical difficulty arose from the accurate determination of the sample masses. The procedure includes preparation of purified sperm nuclei, measurement of the sample mass and direct selenium analysis in the suspensions of the compact sperm nuclei without prior digestion of the matter, using a palladium matrix modifier, a spectrometer with Zeeman background correction and a graphite atomizer with L'vov platform. The detection limit for the determination of selenium was 8.4 pg. The quality control of the results by means of instrumental neutron activation analysis (INAA) showed the reliability of the selenium determination by ETAAS. The procedure proved to be suitable to analyze selenium and thus snGPx in very small amounts of purified human sperm nuclei.     

Determination of cadmium by electrothermal atomic absorption spectrometry after microwave-assisted digestion of animal tissues and sewage sludges

The determination of cadmium in different sample types has been carried out by electrothermal atomization atomic absorption spectrometry with D₂-background correction using a unpyrocoated graphite tube, after pressurized microwave-assisted digestion. Five chemical modifiers [(NH₄)₂HPO₄, Pd(NO)₃)₂, Ni(NO₃)₂, thiourea and Triton X-100] have been assayed and nickel nitrate has been found to be most effective for an accurate determination of cadmium in mussel tissue, pig kidney and sewage sludge. The characteristic mass of the method is of the order of 1 pg and the limit of detection is lower than 0.1 ng/ml.     

Determination of cadmium by electrothermal atomic absorption spectrometry after microwave-assisted digestion of animal tissues and sewage sludges

The determination of cadmium in different sample types has been carried out by electrothermal atomization atomic absorption spectrometry with D(2)-background correction using a unpyrocoated graphite tube, after pressurized microwave-assisted digestion. Five chemical modifiers [(NH(4))(2)HPO(4), Pd(NO)(3))(2), Ni(NO(3))(2), thiourea and Triton X-100] have been assayed and nickel nitrate has been found to be most effective for an accurate determination of cadmium in mussel tissue, pig kidney and sewage sludge. The characteristic mass of the method is of the order of 1 pg and the limit of detection is lower than 0.1 ng/ml.     

Simultaneous determination of manganese and selenium in serum by electrothermal atomic absorption spectrometry

A method for determination of manganese and selenium in serum by simultaneous atomic absorption spectrometry (SIMAAS) is proposed. The samples (30 mul) were diluted (1+3) to 1.0% v/v HNO(3)+0.10% w/v Triton X-100 directly in the autosampler cups. A total of 20 mug Pd+10 mug Mg(NO(3))(2) was used as chemical modifier. The pyrolysis and atomization temperatures for the simultaneous heating program were 1200 and 2300 degrees C, respectively. The addition of an oxidant mixture (15% w/w H(2)O(2)+1.0% v/v HNO(3)) and the inclusion of a low temperature pyrolysis step (400 degrees C) attenuated the build-up of carbonaceous residues onto the integrated platform. An aliquot of 15 mul of the reference or sample solution was introduced into the graphite tube and heated at 80 degrees C; subsequently, 10 mul of oxidant mixture+10 mul of chemical modifier was introduced over that aliquot and the remaining heating program steps were executed. This strategy allowed at least 250 heating cycles for each THGA tube without analytical signal deterioration. The characteristic masses for manganese (6 pg) and selenium (46 pg) were estimated from the analytical curves. The detection limits were 6.5 pg (n=20, 3delta) for manganese and 50 pg (n=20, 3delta) for selenium. The reliability of the entire procedure was checked with the analysis of serum from Seronormtrade mark Trace Elements in Serum (Sero AS) and by addition and recovery tests (97+/-9% for manganese and 96+/-7% for selenium) using five serum samples.     

Low volume microwave digestion for the determination of selenium in marine biological tissues by graphite furnace atomic absorption spectroscopy

A microwave digestion method for the determination of marine biological tissues has been developed to allow determination of selenium in small sample sizes (< 0.1 g). The benefits of this technique include maintaining concentrates in extracts without the subsequent over dilution encountered when using larger vessels, increased sample throughput and reduced loss of volatile material. Freeze dried biological material (< 0.1 g) and nitric acid (1 ml) were placed into 7 ml screw top Teflon vessels which are completely sealed on capping. Two 7 ml vials were placed into larger 120 ml vessels fitted with a Teflon spacer and 10 ml of distilled water. The effects of microwave power and time, and sample mass on selenium recovery from three marine standard reference materials (NIST SRM 1566a Oyster Tissue, NRCC DORM-1 Dogfish Muscle and NRCC TORT-1 Lobster Hepatopancreas) were examined. The optimum conditions: 600 W, 2 min; 0 W, 2 min; 450 W, 45 min, allowed quantitative recoveries of selenium from these and three other standard reference materials (NRCC DOLT-1 Dogfish liver, NIST RM-50 Albacore tuna and IAEA MA-A-2 fish flesh). Studies on sample mass showed that the analysis of sample masses from 0.025 to 0.1 g gave selenium concentrations within the certified range. Six species of selenium: selenite, selenate, selenomethionine, selenocysteine, selenocystamine, and trimethyl selenonium were added to oyster, dogfish, and lobster tissues. Recoveries were near quantitative for all species (94–105%) except trimethyl selenonium (90–101%).     

Determination of selenium in water by electrothermal atomic absorption spectrometry

Summary The electrothermal atomization of selenium has been investigated for the accurate determination of selenium in water samples. Hydrogen seriously affects the atomization temperature of selenium in a molybdenum micro-tube atomizer. The atomization of selenium also suffers from serious interferences caused by salts and other elements. The extraction of selenium diethyldithiocarbamate complex serves to eliminate the interferences from the matrix. The addition of copper allows the suppression of interferences from elements extracted with selenium. The method permits the determination of selenium(IV) and selenium(VI) separately.This research was in part funded by the Ministry of Education, Science and Culture, Japan, under Grant-in-Aid for Scientific Research, for which we express our appreciation.     

Simplified cloud point extraction for the preconcentration of ultra-trace amounts of gold prior to determination by electrothermal atomic absorption spectrometry

A simple and sensitive cloud point extraction method has been developed for the preconcentration of ultra-trace amounts of gold as a prior step to its determination by electrothermal atomic absorption spectrometry. It is based on the extraction of gold in hydrochloric acid medium using the non-ionic surfactant polyethyleneglycolmono-p-nonylphenylether (PONPE 7.5) without adding a chelating agent. The preconcentration of a 50 mL sample solution was thus enhanced by a factor of 200. The resulting calibration graph was linear in the range of 10–200 ng L⁻¹ with a correlation coefficient of 0.9993. The limit of detection (3s) obtained under optimal conditions was 2.0 ng L⁻¹. The relative standard deviation for 10 replicate determinations at a 100 ng L⁻¹ Au level was 3.6%. The method was applied to the ultra-trace determination of gold in water and copper samples.     

Direct determination of selenium in a wild fruit juice by electrothermal atomic absorption spectrometry

A matrix modifier composed of platinum and nickel is proposed for the determination of selenium in a wild fruit juice made from Lantingguo (Vuccinium uliginosam). Five matrix modifiers (copper/nickel, palladium/magnesium, platinum/magnesium, platinum/nickel and platinum/copper) for suppressing the interference effects of seven co-existing elements (potassium, phosphorus, calcium, magnesium, manganese, zinc and iron) in a wild juice were studied and a matrix modifier composed fro;m 10 mug of platinum and 200 mug of nickel was found to give the best performance. Selenium in three juices was determined by electrothermal atomic absorption spectrometry employing the proposed matrix modifier without matrix preseparation. The relative standard deviation was 14% for 0.20 mg l(-1) of selenium. The recoveries were 95-110%. A characteristic mass was 28 pg.     

Determination of trace amounts of manganese in waters by solvent extraction and atomic absorption spectrophotometry

A quick and accurate method of solvent extraction and atomic absorption spectrophotometry for the determination of manganese in waters is described. This method does not require previous treatment of the sample if it contains 3 ppb (or higher) of manganese. The method is based on the extraction of the ion-pair formed between benzohydroxamic acidmanganese complex and trioctylmethylammonium cation in MIBK.     

Arsine generation and determination of trace amounts of arsenic by atomic absorption spectrometry

Arsenic can be determined by atomic absorption spectrometry after reduction to arsine with potassium iodide, tin(II) chloride and zinc powder tablet; the arsine generated is carried into an argon-hydrogen flame by means of argon. Accuracy, precision and speed are satisfactory. Serious interferences arise only from nitric acid, lead, chromium and selenium.     

Direct determination of manganese in microgram amounts of pancreatic tissue by electrothermal atomic absorption spectrometry

Manganese is determined by the direct insertion of freeze-dried biological samples (1–15 μg) or by injection of 2-μl samples of perifusion medium into the graphite furnace. At the most sensitive wavelength (279.5 nm), down to 0.2 pmol of manganese can be measured in the perifusion medium as well as the endogenous manganese in the endocrine and exocrine parts of the pancreas. The latter values were 0.08 ± 0.01 and 0.16 ± 0.01 mmol Mn kg^-1 (dry wt.), respectively. A less sensitive wavelength (403.1 nm) is employed for measuring the larger amounts obtained after incubating the specimens in the presence of manganese(II).     

Comparison of two digestion procedures for the determination of lead in lichens by electrothermal atomic absorption spectrometry

The efficiency of two procedures for the digestion of lichen was investigated using a heating block and a microwave oven. In the open vessels, concentrated nitric acid was added to the samples, left for 1 h, and the addition of 30% (v / v) hydrogen peroxide completed the digestion. In the closed system, the complete digestion was performed using concentrated nitric acid and hydrogen peroxide, reducing the amount of chemicals, time and contamination risk. Both digestion methods gave comparable results, and recoveries were statistically not different. For a lichen sample spiked with 10 μg Pb, the recovery was 111% and 110% using microwave and heating block digestion, respectively, while it was 100% and 103% for a 100 μg Pb spike. For the determination by electrothermal atomic absorption spectrometry samples were diluted 20 times with water and a volume of 20 μL was injected into the graphite furnace without chemical modifier. Pyrolysis and atomization temperatures of 700 °C and 1500 °C, respectively, were used. The characteristic mass was 8.4 ± 0.6 pg for aqueous calibration solutions and 8.9 ± 0.8 pg for samples. Calibration was against matrix matched standards. The recovery test showed some contamination problem with the lowest concentrations in both procedures. The detection limits were 4.4 μg L^− 1 with microwave oven and 5.4 μg L^− 1 with the heating block in the undiluted blank.     

微波消解-原子吸收光谱法测定蚕蛹中的微量元素

分别采用FAAS和GFAAS方法,测定蚕蛹样品中的常见微量元素及有害重金属元素。对微波消解条件和测定方法进行了探讨和优化,并用标准物质贻贝验证,获得较满意的准确度和精密度。方法可用于蚕蛹样品及同类产品的微量元素元素测定。     

Comparison of four microwave digestion methods for the determination of selenium in fish tissue by using hydride generation atomic absorption spectrometry

Four microwave digestion methods of fish tissue for selenium determination by hydride generation atomic absorption spectrometry were compared, in which potassium hexacyanoferrate(III) was chosen as a masking agent for eliminating matrix interferences. The results showed that the methods employing HNO(3)/H(2)O(2), HNO(3)/K(2)S(2)O(8)/H(2)O(2) and HNO(3)/H(3)PO(4)/H(2)O(2) digestion media were unreliable. However, the decomposition using the digestion media of HNO(3)/H(2)SO(4)/H(2)O(2) enabled adequate digestion of fish tissue and retention of selenium in a state amenable for determination. Therefore, the digestion procedures with HNO(3)/H(2)SO(4)/H(2)O(2) media are proposed for the determination of selenium in fish tissue by hydride generation atomic absorption spectrometry. The recoveries of the spiked samples investigated ranged from 90 to 102%. The result obtained from analyzing the NIES CRM No. 6 mussel was in good agreement with the reference value (reference value: 1.5 mug/g; found: 1.45 +/- 0.05 mug/g). The limit of detection for selenium was 0.03 mug/g dry mass for a 100 mg sample. The contents of selenium in local fish species investigated ranged from 0.49 to 2.90 mug/g, and the relative standard deviation for the determination of selenium was less than 8%.     

Comparison of wet microwave digestion methods of plant materials for the determination of metals by flame atomic absorption spectrometry

Microwave closed-system wet digestion procedures for plant samples were examined. Each procedure was tested with samples of tobacco and cabbage, and included digestion by the use of different acids composition, almost complete evaporation of the digest, and then dissolution of the residue in 1% nitric acid. Three microwave digestion programs that varied power, duration, and temperature were used. Closed-vessel reactions followed open-vessel reaction-delay time. Using flame atomic absorption spectrometry on the digests, four or five elements were determined to evaluate effectiveness, precision and accuracy of analytes extraction into solution. After a preliminary study of tobacco digests, the four most effective procedures were chosen, and detailed investigations were carried out on both tobacco and cabbage reference materials. Although all four of the final procedures were accurate, the most precise procedure, with the lowest errors of determination, was using reverse ‘aqua regia’ for tobacco and ‘aqua regia’ for cabbage.     

An improved metal extraction procedure for the determination of trace metals in sea water by atomic absorption spectrometry with electrothermal atomization

A rapid carbamate extraction method with pyrrolidinedithiocarbamate and diethyldithiocarbamate is described for the simultaneous determination of Cd, Co, Cu, Fe, Ni, Pb and Zn in sea water by atomic absorption spectrometry with a graphite atomizer. The metal—carbamate complexes are extracted from 500 ml of sea water into Freon TF and back-extracted into 10 ml of 0.3 M nitric acid. The method has considerable advantages over previously recommended extraction procedures. The metals are transferred to a solution in which their concentrations do not change with time, and which can be easily stored for transportation. The sensitivity is high enough for analysis of open ocean waters.     

Reduction of effects of structured non-specific absorption in the determination of arsenic and selenium by electrothermal atomic absorption spectrometry

The presence of iron and phosphates in biological matrices causes deuterium arc background-correction systems to overcompensate at several arsenic and selenium resonance lines. The addition of platinum as matrix modifier has a significant effect on both the absorbance/time profile of iron and the formation of gaseous phosphate decomposition products. A nickel/platinum matrix modifier is shown effectively to control the problems in the determination of selenium arising both from thermal instability and spectral interferences. The same combination eliminates the spectral interferences found at the arsenic resonance lines. Remaining problems are the thermal stabilization of organometallic arsenic compounds present in biological samples. When radioactived-labelled ⁷⁴As compounds prepared in vivo were applied, none of the tested matrix modifiers (Ni, Cu, Ag, Pd, Zr, Ce, Ce + magnesium nitrate) showed a significant influence on the volatility of arsenic in whole blood and urine from rats.     

石墨炉原子吸收光谱法测定大鼠血清中硒

通过考察不同基体改进剂效果,提出了以硝酸锶和硝酸钯做为混合基体改进剂。建立了用石墨炉原子吸收法测定牛血清和大鼠血清中痕量硒的分析方法。线性范围为0-120ng/mL,硒的检出限为0．095ng／mL,方法用于标准牛血清测定。结果与标准值基本吻合,大鼠血清测定标准加入回收率为102％。     

Hollow fiber supported liquid membrane extraction for ultrasensitive determination of trace lead by portable tungsten coil electrothermal atomic absorption spectrometry

Hollow fiber supported liquid membrane extraction (HF-SLME) was used to separate and enrich trace lead from a large volume of 250 mL water sample to a final tiny volume of 30 μL of 1-octanol, 5 μL of which was inject into a tungsten coil electrothermal atomic absorption spectrometer (W-coil ET-AAS) for determination of lead. Some important parameters that influenced the extraction and determination were investigated in detail, such as the concentration of ammonium pyrrolidine dithiocarbamate (APDC), pH of sample solution, stirring rate, extraction time, pyrolysis current, atomization current, carrier gas flow rate, as well as interferences. Under the optimized conditions, a practical enrichment factor of 499 and a limit of detection (3σ) of 0.2 ng mL^{− 1} were obtained. The calibration curve was linear in the range of 0.5–10 ng mL^{− 1}. The relative standard deviation (RSD) was 5.6% for five measurements of a 4 ng mL^{− 1} lead standard solution. The accuracy of this method was examined by the analysis of certified reference water samples (GBW(E)080398 and GSBZ(E) 50009-88) for lead. Finally, the proposed method was applied to the determination of lead in local tap water, pond water and river water, with recoveries in the range of 96–109% for spiked samples.