Simple mercury fractionation in biological samples by CV AAS following microwave-assisted acid digestion or TMAH pre-treatment

A simple and reliable method to determine total and inorganic mercury in biological certified reference material (CRM) by cold vapor atomic absorption spectrometry (CV AAS) is proposed. After the CRM treatment at room temperature with tetramethylammonium hydroxide (TMAH), inorganic mercury is determined by CV AAS. Total mercury is measured by the same technique, after sample acid digestion in a microwave oven. Organic mercury, basically methylmercury, is obtained by difference. In both procedures, the quartz tube is kept at room temperature. By means of analysis of the following reference materials: pig kidney, lobster hepatopancreas, dogfish liver and mussel tissue, it was clear that the difference between the total and inorganic mercury concentrations agrees with the methylmercury concentration. Only one calibration curve against aqueous standards in acidic medium was carried out for both procedures. The concentrations obtained by both procedures are in agreement with the certified values according to the t-test at a 95% confidence level. The relative standard deviations were lower than 3.0% for digested CRM and 6.0% for CRM treated with TMAH for most of the samples. The limits of detection in the samples were 0.02 µg g^{− 1} and 0.04 µg g^{− 1} for inorganic and total Hg, respectively, since the sample mass for total mercury was half of that for inorganic mercury determination. Simplicity and high efficiency without using chromatographic techniques are some of the qualities of the proposed method, being adequate for fractionation analysis of mercury in biological samples.     

Non-chromatographic speciation analysis of mercury by flow injection on-line preconcentration in combination with chemical vapor generation atomic fluorescence spectrometry

A novel non-chromatographic approach for direct speciation of mercury, based on the selective retention inorganic mercury and methylmercury on the inner wall of a knotted reactor by using ammonium diethyl dithiophosphate and dithizone as complexing agents respectively, was developed for flow injection on-line sorption preconcentration coupled with chemical vapor generation non-dispersive atomic fluorescence spectrometry. With the sample pH kept at 2.0, the preconcentration of inorganic mercury on the inner walls of the knotted reactor was carried out based on the exclusive retention of Hg–DDP complex in the presence of methylmercury via on-line merging the sample solution with ammonium diethyl dithiophosphate solution, and selective preconcentration methylmercury was achieved with dithizone instead of ammonium diethyl dithiophosphate. A 15% (v/v) HCl was introduced to elute the retained mercury species and merge with KBH₄ solution for atomic fluorescence spectrometry detection. Under the optimal experimental conditions, the sample throughputs of inorganic mercury and methylmercury were 30 and 20 h^− 1 with the enhancement factors of 13 and 24. The detection limits were found to be 3.6 ng l^− 1 for Hg²⁺ and 2.0 ng l^− 1 for CH₃Hg⁺. The precisions (RSD) for the 11 replicate measurements of each 0.2 μg l^− 1 of Hg²⁺ and CH₃Hg⁺ were 2.2% and 2.8%, respectively. The developed method was validated by the analysis of certified reference materials (simulated natural water, rice flour and pork) and by recovery measurements on spiked samples, and was applied to the determination of inorganic mercury and methylmercury in biological and environmental water samples.     

Determination of inorganic and total mercury by vapor generation atomic absorption spectrometry using different temperatures of the measurement cell

A simple and inexpensive laboratory-built flow injection vapor generation system coupled to atomic absorption spectrometry (FI-VG AAS) for inorganic and total mercury determination has been developed. It is based on the vapor generation of total mercury and a selective detection of Hg^2 + or total mercury by varying the temperature of the measurement cell. Only the inorganic mercury is measured when the quartz cell is at room temperature, and when the cell is heated to 650 °C or higher the total Hg concentration is measured. The organic Hg concentration in the sample is calculated from the difference between the total Hg and Hg^2 + concentrations. Parameters such as the type of acid (HCl or HNO₃) and its concentration, reductant (NaBH₄) concentration, carrier solution (HCl) flow rate, carrier gas flow rate, sample volume and quartz cell temperature, which influence FI-VG AAS system performance, were systematically investigated. The optimized conditions for Hg^2 + and total Hg determinations were: 1.0 mol l^− 1 HCl as carrier solution, carrier flow rate of 3.5 ml min^− 1, 0.1% (m/v) NaBH₄, reductant flow rate of 1.0 ml min^− 1 and carrier gas flow rate of 200 ml min^− 1. The relative standard deviation (RSD) is lower than 5.0% for a 1.0 μg l^− 1 Hg solution and the limit of quantification (LOQ, 10 s) is 55 ng g^− 1. Certified samples of dogfish muscle (DORM-1 and DORM-2) and non-certified fish samples were analyzed, using a 6.0 mol l^− 1 HCl solution for analyte extraction. The Hg^2 + and CH₃Hg⁺ concentrations found were in agreement with certified ones.     

Determination of inorganic and methylmercury in fish by cold vapor atomic absorption spectrometry and inductively coupled plasma atomic emission spectrometry

Simple and rapid analytical procedures for the determination of Hg²⁺ and methylmercury in fish were proposed after careful optimization of chemical and instrumental parameters for Hg measurement by cold vapor (CV)/hydride generation (HG) atomic absorption spectrometry (AAS) and CV/HG inductively coupled plasma atomic emission spectrometry (ICP-AES). Quantitative extraction of Hg species avoiding any inter-species conversion was achieved by fast microwave assisted solubilization of fish tissue with relatively low amount of tetramethylammonium hydroxide (TMAH) or 6 mol L^− 1 HCl. After careful optimization of chemical parameters selective determination of Hg²⁺ in the presence of excess of methylmercury is attained by using continuous flow CV AAS, 1% m/V SnCl₂ as reductant and 0.1 mol L^− 1 HCl as reaction medium. Simple calibration curve prepared with aqueous standard of Hg²⁺ is recommended for its quantification. Both Hg²⁺ and methylmercury could be determined simultaneously with equal sensitivity by CV/HG ICP-AES directly in the diluted TMAH solution obtained after extraction with 1% m/V NaBH₄ as reductant. Quantification of the sum of Hg²⁺ and methylmercury against calibration curve prepared with aqueous standard of methylmercury is suggested. It should be mentioned that batch hydride generation system with quartz tube heated in air/acetylene flame could also be used for simultaneous determination of both Hg species in fish extracts, with standard additions calibration. The validity of the developed analytical procedures for selective determination of Hg²⁺ and methylmercury (by difference between the total Hg and Hg²⁺) is confirmed by the analyses of certified reference material DOLT-1 and reference material IMEP-20. Very close agreement between certified values and analytical results was found.     

Determination of Cr(VI) in plants by electrothermal atomic absorption spectrometry after leaching with sodium carbonate

The determination of chromium (VI) compounds in plants by electrothermal atomic absorption spectrometry (ET AAS) is proposed based on their leaching with 0.1 M Na₂CO₃. Due to the presence of relatively high amounts of Na₂CO₃ in the resulting samples, the temperature and time of pyrolysis and atomization stages must be optimized to minimize the influence of the matrix. A limit of detection (LOD) for determination of Cr(VI) in plants by ET AAS was found to be 0.024 μg g⁻¹.The concentration of Cr(VI) and total chromium in plants collected in different geographical areas (South Africa and Russia), grown on soils high in chromium was determined. The concentration of Cr(VI) and total Cr in stems and leaves of plants was in the range of 0.04–0.7 μg g⁻¹ and 0.5–10 μg g⁻¹, respectively. The limited uptake of Cr(III) by plants, in comparison to its concentration in soil, can be explained by the very low solubility of natural Cr(III) compounds.Results for the determination of Cr(VI) were confirmed by the analysis of BCR CRM 545 (Cr(VI) in welding dust) with good agreement between certified (39.5 ± 1.3 μg mg⁻¹) and found (38.8 ± 1.2 μg mg⁻¹) values. The total concentration of Cr in plants has also been determined by ET AAS after dry ashing of samples at 650 °C. Results were confirmed by the analysis of BCR CRM 281 (Trace elements in Rye Grass) with good agreement between the found (2.12 ± 0.16 μg g⁻¹) and certified value (2.14 ± 0.12 μg g⁻¹).     

Evaluation of various sample pre-treatment methods for total and inorganic mercury determination in biological certified reference materials by CVAAS technique

Sample preparation methods for non-separation cold vapor atomic absorption spectrometry (CVAAS) sequential inorganic mercury speciation in biological certified reference materials (CRMs) were investigated. The methylmercury concentration was calculated as the difference between total and inorganic mercury. Microwave-assisted decomposition method, and three ultrasonic extraction procedures based on acid leaching with HCl and HCOOH and solubilization with TMAH were employed as sample preparation methods. The replacement of a sample decomposition procedure by extraction prior to analysis by CVAAS, as well as the aspect of speciation analysis is discussed. The limits of detection in the sample were determined as 50 and 10 ng L⁻¹ for inorganic and total mercury, which corresponds to absolute detection limits of 40 and 8 ng g⁻¹ for inorganic and total mercury, respectively. The results were in good agreement with the 95% confidence level t-test of the certified values for total and inorganic mercury in the reference materials investigated. From the analysis of the CRMs, it was evident that the difference between the total and inorganic mercury concentrations agrees with the methylmercury concentration. The relative standard deviation was better than 11% for most of the samples.      

New methodology for anodic stripping voltammetric determination of methylmercury

A novel procedure for trace methylmercury determinations by anodic stripping voltammetry at a gold film electrode is presented. Measurements were performed in a flow system. For selective determination of methylmercury, the Hg²⁺ ions were masked by complexation with DTPA. Hg-DTPA complex is not reduced at the gold film electrode at the potential of methylmercury reduction to the metallic state. The calibration graph was linear from 5 × 10⁻⁹ to 1 × 10⁻⁷ mol L⁻¹ for an accumulation time 600 s. A detection limit (based on 3σ criterion) for methylmercury was 2.3 × 10⁻⁹ mol L⁻¹. The validation of the proposed procedure was made by analyses of human hair certified reference material.     

Determination of lead,cadmium and mercury in blood for assessment of environmental exposure: A comparison between inductively coupled plasma–mass spectrometry and atomic absorption spectrometry

A biomonitoring method for the determination of Pb, Cd, and Hg at background levels in whole blood by inductively coupled plasma-mass spectrometry is described. While this method was optimized for assessing Pb, Cd and Hg at environmental levels, it also proved suitable for assessing concentrations associated with occupational exposure. The method requires as little as 200 μl of blood that is diluted 1 + 49 for direct analysis in the inductively coupled plasma-mass spectrometer. Method performance is compared to well-established AAS methods. Initial method validation was accomplished using National Institute of Standards and Technology (NIST) Standard Reference Material 966, Toxic Metals in Bovine Blood. Method detection limits (3s) are 0.05 μg dl^− 1 for Pb, 0.09 μg l^− 1 for Cd; and 0.17 μg l^− 1 for Hg. Repeatability ranged from 1.4% to 2.8% for Pb; 3% to 10% for Cd; and 2.6% to 8.8% for Hg. In contrast, AAS method detection limits were 1 μg dl^− 1, 0.54 μg l^− 1, and 0.6 μg l^− 1, for Pb, Cd, and Hg, respectively. Further performance assessments were conducted over a 2-year period via participation in four international External Quality Assessment Schemes (EQAS) operated specifically for toxic metals in blood. This includes schemes operated by (a) the New York State Department of Health's Wadsworth Center, Albany, NY, USA (b) L′Institut National de Santé Publique du Québec, Centre de Toxicologie du Québec, Canada, (c) Friedrich-Alexander University, Erlangen, Germany, and (d) the University of Surrey, Guildford, UK Trace Elements scheme. The EQAS data reflect analytical performance for blind samples analyzed independently by both inductively coupled plasma-mass spectrometry and AAS methods.     

Flow injection-chemical vapor generation atomic fluorescence spectrometry hyphenated system for organic mercury determination: A step forward

Monomethylmercury and ethylmercury were determined on line using flow injection-chemical vapor generation atomic fluorescence spectrometry without neither requiring a pre-treatment with chemical oxidants, nor UV/MW additional post column interface, nor organic solvents, nor complexing agents, such as cysteine. Inorganic mercury, monomethylmercury and ethylmercury were detected by atomic fluorescence spectrometry in an Ar/H₂ miniaturized flame after sodium borohydride reduction to Hg⁰, monomethylmercury hydride and ethylmercury hydride, respectively. The effect of mercury complexing agent such as cysteine, ethylendiaminotetracetic acid and HCl with respect to water and Ar/H₂ microflame was investigated.The behavior of inorganic mercury, monomethylmercury and ethylmercury and their cysteine-complexes was also studied by continuous flow-chemical vapor generation atomic fluorescence spectrometry in order to characterize the reduction reaction with tetrahydroborate. When complexed with cysteine, inorganic mercury, monomethylmercury and ethylmercury cannot be separately quantified varying tetrahydroborate concentration due to a lack of selectivity, and their speciation requires a pre-separation stage (e.g. a chromatographic separation). If not complexed with cysteine, monomethylmercury and ethylmercury cannot be separated, as well, but their sum can be quantified separately with respect to inorganic mercury choosing a suitable concentration of tetrahydroborate (e.g. 10^? 5 mol L^? 1), thus allowing the organic/inorganic mercury speciation.The detection limits of the flow injection-chemical vapor generation atomic fluorescence spectrometry method were about 45 nmol L^? 1 (as mercury) for all the species considered, a relative standard deviation ranging between 1.8 and 2.9% and a linear dynamic range between 0.1 and 5 μmol L^? 1 were obtained. Recoveries of monomethylmercury and ethylmercury with respect to inorganic mercury were never less than 91%. Flow injection-chemical vapor generation atomic fluorescence spectrometry method was validated by analyzing the TORT-1 certificate reference material, which contains only monomethylmercury, and obtaining 83 ± 5% of monomethylmercury recovered, respectively. This method was also applied to the determination of monomethylmercury in saliva samples.     

Microwave-radiated synthesis of gold nanoparticles/carbon nanotubes composites and its application to voltammetric detection of trace mercury(II)

Gold nanoparticles/carbon nanotubes (Au-NPs/CNTs) composites were rapidly synthesized by microwave radiation, and firstly applied for the determination of trace mercury(II) by anodic stripping voltammetry (ASV). The structure and composition of the synthesized Au-NPs/CNTs nanocomposites were characterized by transmission electron microscopy (TEM), energy dispersive X-ray spectroscopy (EDX), UV–vis absorption spectroscopy and cyclic voltammetry. Au-NPs/CNTs nanocomposites modified glassy carbon electrode (Au-NPs/CNTs/GCE) exhibited excellent performance for Hg(II) analysis. A wide linear range (5 × 10⁻¹⁰–1.25 × 10⁻⁶ mol/L) and good repeatability (relative standard deviation of 1.84%) were obtained for Hg(II) detection. The limit of detection was found to be 3 × 10⁻¹⁰ mol/L (0.06 μg/L) at 2 min accumulation, while the World Health Organization’s guideline value of mercury for drinking water is 1 μg/L, suggesting the proposed method may have practical utility.     

A multi-syringe flow injection system for the spectrophotometric determination of trace levels of iron in waters using a liquid waveguide capillary cell and different chelating resins and reaction chemistries

A method integrating a long waveguide capillary cell with a preconcentration resin in a multi-syringe flow injection analysis (MSFIA) system for iron determination in waters was developed. The determination of iron is based on a colorimetric reaction and two reagents were tested, ferrozine and ammonium thiocyanate. A liquid waveguide capillary cell (1.0 m pathlength, 550 µm i.d. and 250 µL internal volume) with a preconcentration resin were used to improve the sensitivity of the determination. Two different preconcentration resins were also tested, Chelex 100 and NTA Superflow. The developed method employing the NTA Superflow with ferrozine colorimetric reagent provided a detection limit of 0.05 µg L^− 1 with a linear response up to 8 µg L^− 1 and a sample throughput rate of 12 per hour. The developed system presents low reagents/sample consumptions. The accuracy was assessed using a certified reference water sample.     

Mercury Speciation in Fish by High-Performance Liquid Chromatography (HPLC) and Post-Column Ultraviolet (UV)-Photochemical Vapor Generation (PVG): Comparison of Conventional Line-Source and High-Resolution Continuum Source (HR-CS) Atomic Absorption Spectrometry (AAS)

An ultraviolet-photochemical generator (UV-PVG) capable of post-column on-line transformation of both organic and inorganic mercury species to cold vapor (Hg⁰) with subsequent detection by quartz tube-atomic absorption spectrometry (QT-AAS) was developed. Mercury(II), methylmercury(I), ethylmercury(I), and phenylmercury(I) were successfully detected after separation by reversed-phase high-performance liquid chromatography (RP-HPLC). Two types of AAS detectors were compared. The first was a commonly used line-source instrument while the second was a high-resolution continuum source (HR-CS) AAS. The latter provided better limits of detection: 0.47?µg?L^?1 for Hg(II), 0.84?µg?L^?1 for methylmercury(I), 0.80?µg?L^?1 for ethylmercury(I), and 2.0?µg?L^?1 for phenylmercury(I). The repeatability at 30?μg?L^?1 was 3.6%, 4.1%, 6.2%, and 4.5% for these species (n?=?10). These figures of merit were comparable with those reported for more sensitive atomic fluorescence spectrometry. Nine sample extraction procedures were investigated. Extraction by tetramethylammonium hydroxide and HCl at 75?°C was selected as the only method compatible with the proposed separation and detection steps providing high extraction efficiency and no changes in mercury speciation. The applicability of the proposed high-performance liquid chromatography–ultraviolet-photochemical vapor generation–quartz tube-atomic absorption spectrometry method was demonstrated using fish samples and certified reference materials (CRM) DOLT-4 (dogfish liver) and ERM-CE464 (tuna fish). The results were comparable to those obtained by a reference method based on L-cysteine extraction and high-performance liquid chromatography–inductively coupled plasma-mass spectrometry (HPLC–ICP-MS) determination.     

Ultrafiltration of mixed protein solutions of lysozyme and lactoferrin: role of modified inorganic membranes and ionic strength on the selectivity

Ultrafiltration of either single protein solutions (lysozyme 14,300 g mol⁻¹, pI=11; lactoferrin 80,000 g mol⁻¹, pI=8–9) or mixed protein solution was performed with inorganic membranes (MMCO 300,000 g mol⁻¹, pore radius 14 nm) chemically modified in order to bear either pyrophosphate (PP, anionic) or ethylenediamine (EDA, cationic) groups.The electrophoretic mobility of modified and unmodified zirconia particles fouled with proteins was similar whatever the grafted groups, meaning that the membrane surface was always made of adsorbed proteins during UF. In spite of that, for the UF of lysozyme/lactoferrin mixed solution, the maximum selectivity (S=lysozyme transmission/lactoferrin transmission=165) was observed with the EDA membrane and allowed an instantaneous purity of lysozyme in the permeate close to 100% to be achieved. Such high selectivitiy was mainly due to the negligible transmission of lactoferrin with the membrane modified with the EDA groups in the ionic strength range 0–100 mmol l⁻¹ of NaCl at pH 7 (achieved either for mixed and single solutions).     

Internal standardization in graphite furnace atomic absorption spectrometry: Comparative use of As and Ge to minimize matrix effects on Se determination in milk

Arsenic and germanium have been evaluated as internal standards to minimize matrix effects on the direct determination of selenium in milk by graphite furnace atomic absorption spectrometry (GFAAS) using tubes with integrated platform, pre-treated with W together with Pd as chemical modifier. The efficiency of As and Ge as internal standards for 25 μg L^− 1 Se plus 500 μg L^− 1 As or Ge in diluted (1 + 9 v/v) milk plus 1.0% (v/v) HNO₃ was evaluated by means of correlation graphs plotted from the normalized absorbance signals (n = 20) of internal standard (axis y) versus analyte (axis x). The equations that describe the linear regression were: A^As = − 0.004 ± 0.019 + 1.02 ± 0.019 A^Se (r = 0.9967 ± 0.005); A^Ge = − 0.017 ± 0.015 + 1.01 ± 0.015 A^Se (r = 0.9978 ± 0.004). Samples and reference solutions were automatically spiked with 500 μg L^− 1 Ge or As and 1.0% (v/v) HNO₃ by the autosampler. For 20 μL of aqueous standard solutions, analytical curves in the 5.00–40.0 μg L^− 1 Se range were established using the ratio of Se absorbance to internal standard absorbance (A^Se / A^IS) versus analyte concentration, and good linear correlations were obtained. The characteristic mass was 40 pg Se. Limits of detection were 0.55 and 0.40 μg L^− 1 with As and Ge as the internal standard, respectively. Relative standard deviations (RSD) for a sample containing 25 μg L^− 1 Se were 1.2% and 1.0% (n = 12) using As and Ge, respectively. The RSD without internal standardization was about 6%. The accuracy of the proposed method was evaluated by an addition-recovery experiment and all recovered values were in the 99–105% range with IS and in the 70–80% range without IS. Using Ge as the internal standard, results of analysis of standard reference materials were in agreement with certified values at a 95% confidence level. The selenium concentration for 10 analyzed milk samples varied from 5.0 to 20 μg L^− 1.     

Decomposition of 14C containing organic molecules released from radioactive waste by gamma-radiolysis under repository conditions

Decomposition of ¹⁴C containing organic molecules into an inorganic compound has been investigated by γ-ray irradiation experiments under simulated repository conditions for radioactive waste. Lower molecular weight organic acids, alcohols, and aldehydes leached from metallic waste are reacted with OH radicals to give carbonic acid. A decomposition efficiency that expresses consumption of OH radicals by decomposition reaction of organic molecules is proposed. Decomposition efficiency increases with increasing concentration of organic molecules (1×10⁻⁶–1×10⁻³ mol dm⁻³) and is not dependent on dose rate (10–1000 Gy h⁻¹). Observed dependence indicates that decomposition efficiency is determined by reaction probability of OH radicals with organic molecules.     

Rapid determination of total iodine in Japanese coastal seawater using SF-ICP-MS

A simple and rapid analytical method to measure total iodine in seawater using sector-filed ICP-MS is presented here. The new method avoided tedious and complicated organic iodine decomposing and redox treatment. In addition, no pre-concentration and separation operations are needed. The seawater was diluted 100-fold with 0.5% TMAH prior to SF-ICP-MS analysis. Te was added as internal standard. Due to the high sensitivity of SF-ICP-MS, excellent detection limit of 0.23 ng ml^? 1 in original seawater was obtained. By applying this newly developed method, for the first time, the total iodine concentrations in Japanese coastal seawaters in 14 estuaries were investigated. An average value of 58.26 ± 6.30 ng ml^? 1 (n = 59) for total iodine concentration was obtained for future study on the estimation of sediment–water distribution coefficients and the concentration ratios from water to organisms in Japanese coastal marine environment.     

Pyrohydrolysis of carbon nanotubes for Br and I determination by ICP-MS

Bromine and iodine determination was performed in carbon nanotubes (CNTs) by inductively coupled plasma mass spectrometry (ICP-MS) after sample preparation using pyrohydrolysis. Samples of CNTs (up to 500 mg) were mixed with 750 mg of V₂O₅ and heated at 950 °C during 12.5 min in a quartz tube under water vapor and air. The main operational conditions of pyrohydrolysis (carrier gas, absorbing solution, heating time, sample mass and use of V₂O₅) were evaluated. Accuracy was evaluated using certified reference materials (CRM) with similar matrix and also by comparison of results obtained after digestion of samples by microwave-induced combustion (MIC) and determination by ICP-MS. Agreement with CRM values was higher than 97% for Br and better than 96% in comparison with reference values (MIC/ICP-MS) of Br and I in CNTs samples. The limit of detection of the method for Br and I determination by ICP-MS was 0.05 and 0.004 μg g^? 1, respectively. Using a relatively simple and low cost pyrohydrolysis apparatus up to four samples can be processed per hour. The pyrohydrolysis sample preparation procedure is easy to be performed and provide a clean solution for analysis by ICP-MS, which is very attractive for Br and I control in CNTs.     

Removal of suspended clay from water using transmembrane pressure pulsed microfiltration

Transmembrane pressure pulsing (TPP) uses the frequent and periodic reversal of the transmembrane pressure to reduce flux resistances due to membrane fouling. This study examined the effect of TPP on the microfiltration of simulated drinking water (hydrated aluminum silicate solution). Solutions of kaolin clay (0.1–4.0 μm particles, at an approximate concentration of 500 mg l⁻¹ and a turbidity of 402±17 NTU, 0.5 mM CaCl, 2.0 mM NaHCO₃, pH 7.5–7.8) were microfiltered with polyethersulfone (PES) 0.16 μm microfiltration membranes at an operating pressure of 30 kPa. Crossflow shear rates were varied between 165 and 1490 s⁻¹. Pulse frequency was varied between 0.3×10⁻² and 2 Hz, and pulse amplitude was varied between −3 and −16.5 kPa. It was found that the crossflow shear rates did not significantly effect the non-pulsed permeate flux. An optimum pulse amplitude of about 10 kPa was necessary to maximize the permeate flux for pulse frequencies between 0.3×10⁻² and 2.0 Hz. To insure a reduced solute flux, pulse frequencies less than 0.1 Hz were required. These results indicate that TPP can significantly reduce membrane fouling by inorganic particulate materials that are potentially important constituents of natural waters without negatively impacting the rejection of sub-micron particles due to interactions with material accumulated on the membrane.     

Determination of total mercury and methylmercury in biological samples by photochemical vapor generation

Cold vapor atomic absorption spectrometry (CV-AAS) based on photochemical reduction by exposure to UV radiation is described for the determination of methylmercury and total mercury in biological samples. Two approaches were investigated: (a) tissues were digested in either formic acid or tetramethylammonium hydroxide (TMAH), and total mercury was determined following reduction of both species by exposure of the solution to UV irradiation; (b) tissues were solubilized in TMAH, diluted to a final concentration of 0.125% m/v TMAH by addition of 10% v/v acetic acid and CH₃Hg⁺ was selectively quantitated, or the initial digests were diluted to 0.125% m/v TMAH by addition of deionized water, adjusted to pH 0.3 by addition of HCl and CH₃Hg⁺ was selectively quantitated. For each case, the optimum conditions for photochemical vapor generation (photo-CVG) were investigated. The photochemical reduction efficiency was estimated to be ∼95% by comparing the response with traditional SnCl₂ chemical reduction. The method was validated by analysis of several biological Certified Reference Materials, DORM-1, DORM-2, DOLT-2 and DOLT-3, using calibration against aqueous solutions of Hg²⁺; results showed good agreement with the certified values for total and methylmercury in all cases. Limits of detection of 6 ng/g for total mercury using formic acid, 8 ng/g for total mercury and 10 ng/g for methylmercury using TMAH were obtained. The proposed methodology is sensitive, simple and inexpensive, and promotes “green” chemistry. The potential for application to other sample types and analytes is evident.     

Temperature controlled ionic liquid-dispersive liquid phase microextraction for determination of trace lead level in blood samples prior to analysis by flame atomic absorption spectrometry with multivariate optimization

This paper described a new approach for the preconcentration of lead (Pb²⁺) by temperature controlled ionic liquid-dispersive liquid phase microextraction (TIL-DLME) prior to analyzing by flame atomic absorption spectrometry (FAAS). An ionic liquid (IL) 1-Butyl-3-methylimidazolium hexafluorophosphate [C₄MIM][PF₆] was used as an extractant solvent. The Pb²⁺ was complexed with ammonium pyrrolidinedithiocarbamate (APDC) and then entered into the infinite IL drops at high temperature (> 70 °C). Important variables affecting the microextraction efficiency such as pH, ligand concentration, amount of IL, temperature and incubation time were investigated. The results showed that the coexistent ions had no obvious negative effect on the determination of Pb²⁺. In the optimum experimental conditions, the limit of detection (LOD) and the enhancement factor (EF) were 0.13 μg L^? 1 and 93, respectively. The relative standard deviation (RSD) of 10 μg L^? 1 Pb²⁺ was 4.3%. The developed method was validated by determining Pb²⁺ in certified reference material (CRM) and the results showed that the determined values of Pb²⁺ were in good agreement with the certified value. The proposed method was applied satisfactorily for the preconcentration of Pb²⁺ in acid digested blood samples of children with different respiratory disorders.