Analysis of acrylamide in coffee and dietary exposure to acrylamide from coffee

An analytical method for analysing acrylamide in coffee was validated. The analysis of prepared coffee includes a comprehensive clean-up using multimode solid-phase extraction (SPE) by automatic SPE equipment and detection by liquid chromatography tandem mass spectrometry using electrospray in the positive mode. The recoveries of acrylamide in ready-to-drink coffee spiked with 5 and 10 μg l⁻¹ were 96±14% and 100±8%, respectively. Within laboratory reproducibility for the same spiking levels were 14% and 9%, respectively. Coffee samples (n = 25) prepared twice by coffee machines and twice by a French Press Cafetière coffee maker contained 8±3 μg l⁻¹ and 9±3 μg l⁻¹ acrylamide. Five ready-to-drink instant coffee prepared twice contained 8±2 μg l⁻¹. Hence, the results do not show significant differences in the acrylamide contents in ready-to-drink coffee prepared by coffee machine, French Press or from instant coffee. Medium roasted coffee contained more acrylamide (10 μg l⁻¹) than dark roasted coffee (5 μg l⁻¹). Males aged 35–45 years, drinking on average 1.1 l coffee per day are exposed to the highest doses of acrylamide from coffee. The dietary intake of acrylamide from coffee comprises, on an average, 10 μg day⁻¹ for males and 9 μg day⁻¹ for females aged 35–45 years. Probabilistic modelling of the exposure of Danish consumers (all adults) to acrylamide from coffee shows a mean exposure of 6.5 μg day⁻¹ and a 95 percentile of 18 μg day⁻¹.     

Photoageing of rigid PVC—II. Degradation thickness profiles

Bulk samples of non-photostabilized PVC were exposed in a photochemical reactor equipped with a fluorescent lamp (λ ≥ 300 nm) at 70 °C. After 500 h of exposure, thin (20 μm) slices parallel to the surface were cut with a microtome and analyzed by FTIR and UV spectrophotometry and steric exclusion chromatography. The results reveal the existence of at least three distinct zones: (a) The superficial zone of thickness lower than 100 μm, which is characterized by the predominance of oxidation products and chain scissions; (b) The subcutaneous zone, in the 100–400 μm depth interval characterized by the predominance of the products of HC1 zip elimination (conjugated polyenes) and crosslinking (increase of M_w; and (c) The undegraded core zone beyond 400 μm depth. These characteristics can be partially explained in terms of diffusion controlled oxidation kinetics, but with some peculiarities linked to conjugated polyenes. Among these are the consequences of their photoreactivity and screen effect, and the fact that they are concentrated in fractions of high molecular weight.     

Evaluation of solid-phase micro-extraction coupled to gas chromatography-mass spectrometry for the headspace analysis of volatile compounds in cocoa products

The aroma profile of cocoa products was investigated by headspace solid-phase micro-extraction (HS-SPME) combined with gas chromatography–mass spectrometry (GC–MS). SPME fibers coated with 100 μm polydimethylsiloxane coating (PDMS), 65 μm polydimethylsiloxane/divinylbenzene coating (PDMS-DVB), 75 μm carboxen/polydimethylsiloxane coating (CAR-PDMS) and 50/30 μm divinylbenzene/carboxen on polydimethylsiloxane on a StableFlex fiber (DVB/CAR-PDMS) were evaluated. Several extraction times and temperature conditions were also tested to achieve optimum recovery. Suspensions of the samples in distilled water or in brine (25% NaCl in distilled water) were investigated to examine their effect on the composition of the headspace. The SPME fiber coated with 50/30 μm DVB/CAR-PDMS afforded the highest extraction efficiency, particularly when the samples were extracted at 60 °C for 15 min under dry conditions with toluene as an internal standard. Forty-five compounds were extracted and tentatively identified, most of which have previously been reported as odor-active compounds. The method developed allows sensitive and representative analysis of cocoa products with high reproducibility. Further research is ongoing to study chocolate making processes using this method for the quantitative analysis of volatile compounds contributing to the flavor/odor profile.     

New feature of delayed luminescence: preillumination-induced concavity and convexity in delayed luminescence decay curve in the green alga Pseudokirchneriella subcapitata

A new method for measuring delayed luminescence (delayed fluorescence) employs preillumination and a dark waiting period before normal excitation. The preillumination results in a concavity and a convexity in the decay curve in delayed luminescence in the green alga Pseudokirchneriella subcapitata. Formation of the concavity and the convexity is not affected by excitation wavelength (680 nm and 700 nm). However, the concavity and the convexity progressively decrease as the dark waiting period increases after preillumination. The formation of the concavity and the convexity was inhibited by exposure to the electron transport inhibitors DBMIB (644 μg/L, 2.0 μM) and Antimycin A (55 μg/L, 0.1 μM). Samples exposed to DBMIB exhibited noticeable reduction in the concavity, whereas samples exposed to Antimycin A exhibited pronounced reduction in the convexity. There is a possibility that the formation and disappearance of the concavity and the convexity are due to the reduction–oxidation state of the plastoquinone pool and the cyclic electron transport. We expect this method being useful in evaluating the effects of chemicals (particularly toxic chemicals) on photosynthetic reactions, and the method may also help to resolve questions regarding the source of long delayed luminescence.     

Flow injection on-line dilution for zinc determination in human saliva with electrothermal atomic absorption spectrometry detection

An automated method is described for the determination of zinc in human saliva by electrothermal atomic absorption spectrometry (ET AAS) after on-line dilution of samples with a significant reduction of sample consumption per analysis (<0.4 mL including the dead volume of the system). In order to fulfill this aim without changing the sample transport conduits during the experiments, a flow injection (FI) dilution system was constructed. Its principal parts are: one propulsion device (peristaltic pump, PP) for either samples, standards or washing solution all located in an autosampler tray and for the surfactant solution (Triton X-100) used as diluent, and a two-position time based solenoid injector (TBSI₁) which allowed the introduction of 10 μL of either solution in the diluent stream. To avoid unnecessary waste of samples, the TBSI₁ also permitted the recirculation of the solutions to their respective autosampler cups. The downstream diluted solution fills a home made sampling arm assembly. The sequential deposition of 20 μL aliquots of samples or standards on the graphite tube platform was carried out by air displacement with a similar time based solenoid injector (TBSI₂). The dilution procedure and the injection of solutions into the atomizer are computer controlled and synchronized with the operation of the temperature program. Samples or standards solutions were submitted to two drying steps (at 90 and 130 °C), followed by pyrolysis and atomization at 700 and 1700 °C, respectively. The aqueous calibration was linear up to 120.0 μg L⁻¹ for diluted standard solutions/samples and its slope was similar (p > 0.05) to the standard addition curve, indicating lack of matrix effect. The precision tested by repeated analysis of real saliva samples was less than 3% and the detection limit (3σ) was of 0.35 μg L⁻¹. To test the accuracy of the proposed procedure, recovery tests were performed, obtaining mean recovery of added zinc of 97.8 ± 1.3%. Furthermore, Zn values estimated by the procedure developed in this work were compared with those obtained by a standard addition flame-AAS method applied to 20 randomly selected saliva samples. No significant differences (p > 0.05) were obtained between the two methods. Zinc levels in saliva samples from 44 healthy volunteers, 15 male and 29 female, with ages between 20 and 51 years (mean 30.50 ± 9.14 years) were in the range 22–98 μg L⁻¹ (mean of 55 ± 17 μg L⁻¹), similar to some and different from others reported in the literature. It was found that zinc values for male were statistically higher (p = 0.006) than for female.     

Automatic in-tube SPME and fast liquid chromatography: a cost-effective method for the estimation of dibuthyl and di-2-ethylhexyl phthalates in environmental water samples

A 80-cm length commercially available capillary coated with 95% polydimethylsiloxane and 5% polydiphenylsiloxane (TBR-5) was employed to carry out on-line extraction and preconcentration of dibuthyl phthalate (DBP) and di-2-ethylhexyl phthalate (DEHP) in the chromatographic system. The coated capillary was placed between the sample injection loop and the injection needle of an autosampler. Variables affecting the automatic in-tube solid-phase microextraction (SPME) were optimized. A Genesis C₁₈ (5 cm × 4.6 mm i.d., 4 μm particle size) was employed as analytical column. The achieved limits of detection by use of diode array detection were 1 and 2.5 μg L⁻¹, respectively. The proposed conditions have been applied to determine those compounds at low ppb levels (≤250 μg L⁻¹) in aqueous samples. No matrix effect was found, and recoveries between 85 and 115% were obtained. The precision of the method was good, and the achieved intra- and inter-day variation coefficients were between 5 and 20%. The analysis time per sample was 20 min and any off-line pre-treatment of the samples was needed. The taken sample volume was 100 μL. Data on the application of the described method to the analysis of different water samples are presented.     

Sub-picomole high-performance liquid chromatographic/mass spectrometric determination of glutathione in the maize (Zea mays L.) kernels exposed to cadmium

Changes in fresh weight, total protein amounts (Bradford’s method), cadmium concentration (DPASV) and glutathione content (HPLC/MS) were studied in maize kernels cultivated for 5 days at three different cadmium concentrations (0, 10 and 100 μmol l⁻¹ CdCl₂). A highly sensitive HPLC/MS method was used for the determination of glutathione on a reversed-phase Atlantis dC₁₈ chromatographic column (150 mm×2.1 mm, 3 μm particle size). An isocratic mode with acetonitrile–0.01% TFA (5:95, flow rate 0.1 ml min⁻¹ and 30 °C) was applied. The m/z spectra and the data for the selected ion monitoring (SIM) mode were recorded at m/z for glutathione 308→179. Cadmium concentration was measured by a differential pulse adsorptive stripping voltammetry (DPASV) after deposition on a hanging mercury drop electrode (HMDE) at potential −0.7 V (accumulation time 180 s, acetate buffer of pH 3.6, 22 °C). An AUTOLAB with a VA-Stand 663 and a three-electrode system consisting of the HMDE as a working electrode with area 0.4 mm², an Ag/AgCl/3 mol l⁻¹ KCl as a reference electrode and a Pt-wire as an auxiliary electrode was employed. The maize kernels exposed to the highest cadmium concentration (100 μmol l⁻¹) germinated formerly and much better. A rapid increase of the fresh weight probably relates with more intensive uptake of water in order to decrease cadmium concentration. An intensive preservation of homeostasis of Cd²⁺ ions in the germinating plants by defending mechanisms might explain differences of uptake rate of cadmium. The linear increase of GSH content with the exposure time at all studied concentration suggests the defending mechanisms might be triggered by concentrations of a heavy metal.     

Radiation resistance of GaAs–AlGaAs heterostructures doped with isovalent and rare-earth elements

When GaAs–Si and GaAs–AlGaAs heterostructures are exposed to γ-quanta, radiation stimulated ordering is observed. However, the gettering efficiency in such systems falls for layer widths more than 1 μm. For this reason we seek effective methods of radiation resistance improvement of materials in which one would expect point radiation defects to be gettered not only at defect boundaries, but also in the active layer volume.

S.i.GaAs–s.i.Al_xGa_1−xAs–nGaAs : Te heterostructures are presented with epitaxial layers (doped with Yb or undoped), obtained by means of LPE (liquid-phase epitaxy). The electron concentration in nGaAs was found to be (1–3)×10¹⁸ cm⁻³ for widths 1–3 μm. The samples were exposed to ⁶⁰Co γ-quanta with doses of 10⁵–10⁷ rad.

Investigations of irradiated samples by means of low-temperature (4.2 K) photoluminescence have shown considerable decrease of exciton halfwidth in the boundary spectra of nGaAs : Te : Yb epitaxial layers in comparison with nGaAs : Te layer spectra. This is caused by background impurity gettering which happens on the s.i.Al_xGa_1−xAs–nGaAs heteroboundaries as well as in deformed regions in the epitaxial layer volume. Formation of such regions is caused by the difference between the covalent radii of Yb atoms and GaAs lattice atoms. The maximum effect of radiation stimulated gettering of dopants in nGaAs epitaxial layers is observed for Yb concentrations which are equal to 10⁻⁴–10⁻⁵ atomic fractions in a solution-melt.

It is determined that the deformed regions in epitaxial layer volumes and heteroboundaries could be efficient drains for point radiation defects which form under radiation exposure. The investigations carried out showed that the doping of an epitaxial layers by rare-earth impurities provides considerable improvement in forming radiation resistant III–V materials.     

Sequential injection sample introduction microfluidic-chip based capillary electrophoresis system

A sequential injection micro-sample introduction system was coupled to a microfluidic-chip based capillary electrophoresis system through a split–flow sampling interface integrated on the micro-chip. The microfluidic system measured 20×70×3 mm in dimension, and was produced using a non-lithographic approach with components readily available in the analytical laboratory. In the H-configuration channel design the horizontal separation channel was a 75 μm I.D.×60 mm quartz capillary, with two vertical side arms produced from plastic tubing. The conduits were embedded in silicon elastomer with a planar glass base. Sequential introduction of a series of samples with about 2.5% carryover was achieved at 48 h⁻¹ throughput with samples containing a mixture of fluorescein isothiocyanate (FITC)-labeled amino acids using SI sample volumes of 3.3 μl and carrier flow-rate of 2.0 ml min⁻¹. Baseline separation was achieved for FITC-labeled arginine, phenylalanine, glycine and FITC (laser induced fluorescence detection) in sodium tetraborate buffer (pH 9.2) within 8–80 s, at separation lengths of 25–35 mm and electrical field strengths of 250–1500 V cm⁻¹, with plate heights in the 0.7–3 μm range.     

Electroless Ni-plating on PTFE fine particles

A Ni electroless plating process was used with polytetrafluoroethylene (PTFE) fine particles (25–500 μm). Using nonionic hydrocarbon surfactant, PTFE particles were dispersed in the plating bath. The PTFE hydrophobicity was sufficiently high that Ni was deposited partly on the PTFE surface in the initial step. The Ni-PTFE particles were formed into the Ni-PTFE plate by heat treatment at 350 °C after pressing. The Ni-PTFE plate had electrical conductivity and gas permeability, which were influenced by the pore distribution in the plate. Pores with 1 μm diameter might be especially important to impart high gas permeability to the Ni-PTFE plate.     

Effect of laser modified surface microtopochemistry on endothelial cell growth

The introduction of microelectronics technology in the area of biological sciences has brought forth previously unforeseeable applications such as DNA or protein biochips, miniaturized, multiparametric biosensors for high performance multianalyte assays, DNA sequencing, biocomputers, and substrates for controlled cell growth (i.e. tissue engineering). We developed and investigated a new method using “cold” excimer laser beam technology combined with microlithographical techniques to create surfaces with well defined 3D microdomains in order to delineate critical microscopic surface features governing cell–material interactions. Microfabricated surfaces with microgrooves 30–3 μm deep, 10–1 μm wide spaced 30 μm apart were obtained with micron resolution, by “microsculpturing” polymer model surfaces using a computer controlled laser KrF excimer beam coupled with a microlithographic projection technique. The laser beam after exiting a mask was focused onto the polymer target surface via an optical setup allowing for a 10-fold reduction of the mask pattern. Various 3D micropatterned features were obtained at the micron level. Reproducible submicron features could also be obtained using this method. Subsequently, model human umbilical endothelial cells (HUVEC) were cultured on the laser microfabricated surfaces in order to study the effects of specific microscopic surface features on cell deposition and orientation. Cell deposition patterns were found to be microstructure dependant, and showed cell orientation dependency for features in the cell range dimension, a behaviour significantly different from that of a previously studied cell model (osteoprogenitor cell). This model may be a promising in so far as it is very rapid (a time frame less than a second per square centimeter of micropatterned surface) and provides further insights into the effects of surface microtopography on cell response with possible applications in the field of biosensors, biomedical and/or pharmaceutical engineering sciences.     

Kinetic spectrophotometric method for rapid determination of trace formaldehyde in foods

A simple and sensitive kinetic-spectrophotometric method was developed for the determination of ultra trace amount of formaldehyde in food samples. The method was based on the oxidation of rhodamine B (RhB) by potassium bromate in sulfuric acid medium (formaldehyde as catalyst). The reaction was monitored by measuring the decrease in absorbance of the dye at 515 nm after 6 min. The developed method allowed the determination of formaldehyde in the range of 10–100 μg L⁻¹ with good precision, accuracy and the detection limit was down to 2.90 μg L⁻¹. The relative standard deviations for the determination of 10 and 60 μg L⁻¹ of formaldehyde were 3.0% and 1.9% (n = 10), respectively. The method was found to be sensitive, selective and was applied to the determination of formaldehyde in foods with satisfactory results.     

A biosensor based on graphite epoxy composite electrode for aspartame and ethanol detection

A gelatin membrane with carboxyl esterase and alcohol oxidase was subsequently integrated onto the surface of a graphite epoxy composite electrode (GECE). The developed biosensors showed linearity in the range of 2.5–400 μM for aspartame and 2.5–25 μM for ethanol with response times of 170 and 70 s for each analyte, respectively. The resulting bienzyme biosensor was used for aspartame detection in diet coke samples and ethanol detection in beer and wine samples. From the obtained results, it can be concluded that the developed biosensor is a selective, practical and economic tool for aspartame and ethanol detection in real samples.     

Supported liquid membranes for the determination of vanillin in food samples with amperometric detection

A supported liquid membrane system has been developed for the extraction of vanillin from food samples. A porous PTFE membrane is impregnated with an organic solvent, which forms a barrier between two aqueous phases. The analyte is extracted from a donor phase into the hydrophobic membrane and then back extracted into a second aqueous solution, the acceptor. The determination (100–1400 μg ml⁻¹ vanillin) was performed using a PVC-graphite composite electrode versus Ag/AgCl/3MKCl at +0.850 V placed in a wall-jet flow cell as amperometric detector. The solid sample is directly placed in the membrane unit without any treatment, and the analyte was extracted from the sample, passes through the membrane and conduced to the flow cell by the acceptor stream. The limit of detection (3σ) was 44 μg ml⁻¹. The method was applied to the determination of vanillin (9–606 μg g⁻¹) in food samples.     

Chemically surface-modified carbon nanoparticle carrier for phenolic pollutants: Extraction and electrochemical determination of benzophenone-3 and triclosan

Chemically surface-modified (tosyl-functionalized) carbon nanoparticles (Emperor 2000 from Cabot Corp.) are employed for the extraction and electrochemical determination of phenolic impurities such as benzophenone-3 (2-hydroxy-4-methoxybenzophenone) or triclosan (5-chloro-2-(2,4-dichlorophenoxy)phenol). The hydrophilic carbon nanoparticles are readily suspended and separated by centrifugation prior to deposition onto suitable electrode surfaces and voltammetric analysis. Voltammetric peaks provide concentration information over a 10–100 μM range and an estimated limit of detection of ca. 10 μM (or 2.3 ppm) for benzophenone-3 and ca. 20 μM (or 5.8 ppm) for triclosan.

Alternatively, analyte-free carbon nanoparticles immobilized at a graphite or glassy carbon electrode surface and directly immersed in analyte solution bind benzophenone-3 and triclosan (both with an estimated Langmuirian binding constants of K ≈ 6000 mol⁻¹ dm³ at pH 9.5) and they also give characteristic voltammetric responses (anodic for triclosan and cathodic for benzophenone-3) with a linear range of ca. 1–120 μM. The estimated limit of detection is improved to ca.5 μM (or 1.2 ppm) for benzophenone-3 and ca. 10 μM (or 2.3 ppm) for triclosan. Surface functionalization is discussed as the key to further improvements in extraction and detection efficiency.     

Determination of dioxopromethazine hydrochloride by capillary electrophoresis with electrochemiluminescence detection

The paper presents a rapid method for the determination of dioxopromethazine hydrochloride (DPZ), an antihistamine drug, by the capillary electrophoresis with electrochemiluminescene detection (CE–ECL) using tris(2,2′-bipyridyl)ruthenium(II) (Ru(bpy)₃²⁺) reagent. This CE–ECL detection method has high sensitivity, good selectivity and reproducibility for DPZ analysis. Under the optimized conditions: separation capillary, 38 cm length (25 μm i.d.); sample injection, 10 s at 8 kV; separation voltage, 12.5 kV; running buffer, 20 mmol L⁻¹ sodium phosphate of pH 6.0; detection potential, 1.15 V; 50 mmol L⁻¹ of phosphate buffer (pH 7.14) containing 5 mmol L⁻¹ of Ru(bpy)₃²⁺ in ECL detection cell, the detection limit of DPZ was 0.05 μmol L⁻¹ (S/N = 3). The linear range extended from 5 to 100 μmol L⁻¹. The linear curve obtained was Y = 181.62 + 9.28X with a correlation coefficient of 0.9970. The relative standard deviations of the ECL intensity and the migration time for six continuous injections of 5 μmol L⁻¹ DPZ were 3.7% and 0.92%, respectively. The CE–ECL method was applied to analyze DPZ in real samples including tablets, rat serum and human urine, and satisfactory results were obtained without interference from samples matrix. The CE–ECL technique was proved to be a potential method for the detection of DPZ in clinic analysis.     

As, Cd, Cr, Ni and Pb pressurized liquid extraction with acetic acid from marine sediment and soil samples

Rapid leaching procedures by Pressurized Liquid Extraction (PLE) have been developed for As, Cd, Cr, Ni and Pb leaching from environmental matrices (marine sediment and soil samples). The Pressurized Liquid Extraction is completed after 16 min. The released elements by acetic acid Pressurized Liquid Extraction have been evaluated by inductively coupled plasma-optical emission spectrometry. The optimum multi-element leaching conditions when using 5.0 ml stainless steel extraction cells, were: acetic acid concentration 8.0 M, extraction temperature 100 °C, pressure 1500 psi, static time 5 min, flush solvent 60%, two extraction steps and 0.50 g of diatomaceous earth as dispersing agent (diatomaceous earth mass/sample mass ratio of 2). Results have showed that high acetic acid concentrations and high extraction temperatures increase the metal leaching efficiency. Limits of detection (between 0.12 and 0.5 μg g^− 1) and repeatability of the over-all procedure (around 6.0%) were assessed. Finally, accuracy was studied by analyzing PACS-2 (marine sediment), GBW-07409 (soil), IRANT-12-1-07 (cambisol soil) and IRANT-12-1-08 (luvisol soil) certified reference materials (CRMs). These certified reference materials offer certified concentrations ranges between 2.9 and 26.2 μg g^− 1 for As, from 0.068 to 2.85 μg g^− 1 for Cd, between 26.4 and 90.7 μg g^− 1 for Cr, from 9.3 to 40.0 μg g^− 1 for Ni and between 16.3 and 183.0 μg g^− 1 for Pb. Recoveries after analysis were between 95.7 and 105.1% for As, 96.2% for Cd, 95.2 and 100.6% for Cr, 95.7 and 103% for Ni and 94.2 and 105.5% for Pb.     

Preparation of a pinhole-free Pd–Ag membrane on a porous metal support for pure hydrogen separation

A pinhole-free palladium membrane with a thickness of 3 μm has been prepared on the surface of a porous sintered stainless steel tube coated with a thin silver layer as a diffusion barrier. Filling of aluminum hydroxide gel in the surface pores of the tube is effective in preventing defect formation during electroless plating of the palladium layer, while the volume of the hydroxide beneath the membrane decreases greatly upon thermal treatment up to 500 °C. The hydrogen flux at 400–500 °C is reasonably proportional to the pressure difference between the two sides of the membrane. Addition of a 2 μm Pd_0.8Ag_0.2 alloy layer on the membrane by electroplating does not greatly decrease the hydrogen permeability.     

Trace analysis of chlorobenzenes in water samples using headspace solvent microextraction and gas chromatography/electron capture detection

In the present work, a rapid method for the extraction and determination of chlorobenzenes (CBs) such as monochlorobenzene, 1,2-dichlorobenzene, 1,3-dichlorobenzene, 1,4-dichlorobenzene, 1,2,3-trichlorobenzene and 1,2,4-trichlorobenzene in water samples using the headspace solvent microextraction (HSME) and gas chromatography/electron capture detector (ECD) has been described. A microdrop of the dodecane containing monobromobenzene (internal standard) was used as extracting solvent in this investigation. The analytes were extracted by suspending a 2.5 μl extraction drop directly from the tip of a microsyringe fixed above an extraction vial with a septum in a way that the needle passed through the septum and the needle tip appeared above the surface of the solution. After the extraction was finished, the drop was retracted back into the needle and injected directly into a GC column. Optimization of experimental conditions such as nature of the extracting solvent, microdrop and sample temperatures, stirring rate, microdrop and sample volumes, the ionic strength and extraction time were investigated. The optimized conditions were as follows: dodecane as the extracting solvent, the extraction temperature, 45 °C; the sodium chloride concentration, 2 M; the extraction time, 5.0 min; the stirring rate, 500 rpm; the drop volume, 2.5 μl; the sample volume, 7 ml; the microsyringe needle temperature, 0.0 °C. The limit of detection (LOD) ranged from 0.1 μg/l (for 1,3-dichlorobenzene) to 3.0 μg/l (for 1,4-dichlorobenzene) and linear range of 0.5–3.0 μg/l for 1,2-dichlorobenzene, 1,3-dichlorobenzene and from 5.0 to 20.0 μg/l for monochlorobenzene and from 5.0 to 30 μg/l for 1,4-dichlorobenzene. The relative standard deviations (R.S.D.) for most of CBs at the 5 μg/l level were below 10%. The optimized procedure was successfully applied to the extraction and determination of CBs in different water samples.     

Evaluation of a synergetic effect between Rh as permanent chemical modifier and acetylacetone as complexing agent in Sc determination in sediment slurry samples by ETAAS

In the present work, scandium was determined in sediment slurry samples (from three different rivers) by electrothermal atomic absorption spectrometry (ETAAS). Slurries were prepared by weighting 100 mg of dry sediment samples (≤53 μm particle sizes) and adding 6 ml of HCl:HNO₃:HF (3:1:2, v/v). Accurate results were only possible due to the synergetic effect between Rh as permanent chemical modifier and acetylacetone (Acac) as complexing agent. The same platform was used for 400 heating cycles. The performance of the chemical modification was evaluated by using scanning electron microscopy (SEM), synchrotron radiation X-ray fluorescence (SRXRF) and some figures of merit (precision and detectability). The best analytical conditions were attained using 1500 and 2550 °C as pyrolysis and atomization temperatures. The scandium content in the liquid phase of the slurries ranged from 61 to 73%, thus indicating, in this study, that both liquid and solid phases play an important role in slurry analyses. An amount of 5.0–20.0 μg l⁻¹ Sc linear range as well as LOD and LOQ of 0.19 and 0.62 μg l⁻¹, respectively, were obtained under these conditions. The accuracy was checked by using microwave-assisted decomposition, and the results compared to those obtained with the proposed methodology (slurry analysis). By checking both sets of the results, there is no statistical difference at the 95% confidence levels.