Solid-Phase Extraction and Spectrophotometric Determination of Trace Amounts of Mercury in Natural Samples

A sensitive and selective solid phase spectrophotometric method for the determination of trace amounts of inorganic mercury is described. Hg²⁺ was sorbed on a silica gel-packed column as an Hg²⁺–N,N-bis(2-mercaptophenyl)ethanediamide (H₂L) complex. The Hg²⁺ complex was eluted from the column using 7mL of acetone. Various parameters including pH, column flow rate, and ligand concentration were optimized. The complex was found to obey Beers law from 2.3 to 73.7µgmL^–1 within the optimum range when the preconcentration factor was two. The effective molar absorption coefficient at 523nm was 1.17×10³Lmol^–1cm^–1 at 523nm. The concentration limits in Beers law dropped from 0.09 to 2.95µgmL^–1 within the optimum range when the preconcentration factor was 50. The relative standard deviation at a concentration level of 5µgmL^–1 Hg²⁺ (9 repetitive determinations) was 1.6%. The detection limits are 0.34µgmL^–1 and 0.015µgmL^–1 when the preconcentration factors are 2 and 50, respectively. The method has been used for routine determination of trace levels of Hg²⁺ in natural waters. The potential application of this method for the removal of Hg²⁺ from natural samples (sea water and lake water) spiked with 100ngmL^–1 of Hg²⁺ was studied. In order to validate the proposed method, LGC 6156 (harbour sediment – extractable metals) was analysed by this method. The results proved that excellent extraction of Hg²⁺ from both natural water samples was obtained by solid phase extraction using N,N-bis(2-mercaptophenyl) ethanediamide.     

Determination of Dextromethorphan and Dextrorphan in Human Urine by High Performance Liquid Chromatography for Pharmacogenetic Investigations

The aim of the present study was to develop a sensitive method to measure dextromethorphan and dextrorphan in urine by HPLC to support pharmacogenetic studies in ethnic groups. Linearity was assessed in the range: 0.015–10 g mL^–1 for dextromethorphan and 1-10 g mL^–1 for dextrorphan. Inter and intra-day coefficients of variation were < 10%. Limits of detection and quantitation were 0.003 g mL^–1 and 0.015 g mL^–1 for dextromethorphan and 0.24 g mL^–1 and 1.0 g mL^–1 for dextrorphan, respectively. The method is reliable in helping determine the phenotype of Mexican ethnic groups using model drugs such as dextromethorphan.     

Determination of 6-amino-2,2-dimethyl-1,3-dioxepan-5-ol by postcolumn derivatization witho-phthalaldehyde/2-mercapto-ethanol after ion-pair chromatography

Summary A high-performance liquid chromatographic method is discribed for the determination of 6-amino-2,2-dimethyl-1,3-dioxepan-5-ol using Spherisorb ODS II stationary phase and mobile phase 30:70 (v/v) methanol: aqueous 1-octane sulfonic acid. Detection was fluorimetric following postcolumn derivatization with o-phthaladehyde/2-mercaptoethanol. The procedure was applied to the analysis of aqueous solutions and microcrystalline suspensions in liquid paraffin, prepared for investigation of the toxicological profile. The method was validated for selectivity, linearity of detector response, repeatability, limit of detection and quantitation. The HPLC method was selective. The instrumental limit of detection was 0.5 ng per injection (0.05 g mL^–1). The method detection limits were 0.5 g mL^–1 aqueous solution and 5 g mL^–1 liquid paraffin suspension, the quantitation limit 0.05 mg mL^–1 aqueous solution and 1.0 mg mL^–1 liquid paraffin. Linearity was within 0.94–47.1 g mL^–1. Intra-assay accuracy accounted for 99–100% in the range 0.05–226 mg mL^–1 aqueous solution, intra-assay precision for 2% (C.V.). For microcrystalline liquid paraffin suspensions with 1 and 250 mg mL^–1 99 and 109% was found for intra-assay accuracy. Intra-assay precision was 5% (C.V.). Reliable results over a wide concentration range can be obtained. The procedure is considered valid for determination of the analyte in aqueous solution or microcrystalline paraffin oil suspensions.     

Energy Transfer Electrogenerated Chemiluminescence for the Determination of Sulfite

A simple and novel electrogenerated chemiluminescence (ECL) method for the determination of sulfite has been developed based on the energy transfer ECL process. It was found that a weak ECL signal of sulfite was electrochemically generated on a platinum electrode in neutral aqueous solution. The signal was strongly enhanced by rhodamine B as an energy receptor and further enhanced by the neutral surfactant Tween 80. In 0.10M phosphate buffer solution (pH=7.5) containing 2.0×10^–6gmL^–1 rhodamine B and 0.4% (v/v) Tween 80, the ECL response to the concentration of sulfite at a potential of 0.82V was linear over a range of 1.0×10^–7gmL^–1 to 8.0×10^–6gmL^–1, and the detection limit was 5×10^–8gmL^–1. The relative standard deviation (n=11, 1.0×10^–6gmL^–1) was 3.8%. The proposed method has been successfully applied to the determination of sulfite in pharmaceutical injections and white sugar samples.     

Flame Atomic Absorption Spectrometric Determination of Gold and Palladium Using Microcolumn On-line Preconcentration and Separation

A microcolumn on-line preconcentration and separation system was developed for the flame atomic absorption spectrometric (FAAS) determination of trace levels of gold and palladium. The analytes were selectively adsorbed onto the microcolumn packed with 2-mercaptothiazole immobilized silica gel (MBTSG) in an acidity range of 0.1 to 6.0M HCl at a sampling flow rate of 4.0mLmin^–1. The analytes adsorbed could be desorbed by a thiourea solution with a flow rate of 2.0mLmin^–1. Most of the common coexisting metal ions at a concentration of 25.0mgmL^–1 and anions at a concentration of 50.0mgmL^–1 did not interfere with the preconcentration and determination of Au and Pd. The limits of detection (LOD), defined as three times the standard deviation of the blank (3), of Au and Pd are 10ngmL^–1 and 26ngmL^–1, respectively, with a preconcentration time of 60s. The relative standard deviation (RSD) is about 2.0% for 0.20µgmL^–1 Au and 0.30µgmL^–1 Pd. With a sample loading time of 30min, 6.7ngmL^–1 Au and 10ngmL^–1 Pd can be preconcentrated quantitatively. A geological sample, an anode slime and a secondary nickel alloy were successfully determined with the proposed method, and the results obtained showed good agreement with the certified values.Received December 23, 2002; accepted May 14, 2003 Published online August 8, 2003     

Characterization of airborne particulates by laser microprobe mass analysis

Summary Laser microprobe mass analysis (LAMMA) was applied to characterize aerosol particles collected and separated from 16m to 0.06m by a low pressure cascade impactor. Positive ion LAMMA spectra showed characteristic molecular peaks such as PbCl⁺, a series of Si₂O⁺–Si₂O₄ ⁺ and NaAl₂Si₂O₂ ⁺–NaAl₂Si₂O₅ ⁺, and TiO⁺ in 0.06–0.12m, 0.5–1m and 4–8m fraction, respectively. In the negative ion LAMMA spectra, it was observed that the fragment peaks of sulfate ions were deficient above 2m and those of nitrate ions were deficient under 2m. LAMMA allows remarkable insights into the chemical nature of aerosol particles.

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Charakterisierung luftgetragener Teilchen durch Laser-Microprobe-Massenspektrometrie

Zusammenfassung Laser-Microprobe-Spektrometrie (LAMMS) wurde zur Analyse atmosphärischen Aerosols herangezogen, welches im Korngrößenbereich zwischen 16m und 0.06m mit einem Niederdruckkaskadenimpaktor fraktioniert gesammelt wurde. Positive LAMMS-Spektren zeigten charakteristische molekulare Peaks, wie etwa PbCl⁺, eine Serie von Si₂O⁺–Si₂O₄ ⁺ und NaAl₂Si₂O₂ ⁺–NaAl₂Si₂O₅ ⁺, sowie TiO⁺ in der 0,06–0,12-m,- 0,5–1–m- bzw. 4–8-m-Fraktion. In den negativen LAMMS-Spektren konnten über 2m keine Fragmentpeaks für Sulfationen, unter 2m. keine für Nitrationen beobachtet werden. LAMMS ermöglicht eine bemerkenswerte Einsicht in die chemische Natur von Aerosolteilchen.

     

Simple and Sensitive Assay for Nucleic Acids Using their Quenching Effect on the Chemiluminescence Reaction Between Luminol and Hydrogen Peroxide with Manganese-Tetrasulfonatophthalocyanine as a New Catalyst

The manganese-tetrasulfonatophthalo-cyanine (MnTSPc) catalyzed luminol-hydrogen peroxide chemiluminescence (CL) system can be quenched in the presence of nucleic acids. A new and highly sensitive CL quenching method for determining nucleic acids in aqueous solutions has been developed. Under optimum conditions, linear relationships were found between the quenched intensity of CL and the concentration of nucleic acids in the range 0.10–2.0µgmL^–1 for calf thymus DNA and 0–1.6µgmL^–1 for fish sperm DNA. The limits of detection were 14.8ngmL^–1 for calf thymus DNA and 21.7ngmL^–1 for fish sperm DNA. The relative standard deviation (RSD) of nine replicate measurements is 1.4% for 1.0µgmL^–1 calf thymus DNA. The method was applied to the analysis of nucleic acids in synthetic samples and the results are satisfactory.Received December 2, 2002; accepted June 2, 2003 published online September 1, 2003     

The composition of volatile and particulate hydrocarbons in urban air

Summary The hydrocarbon composition of the particle and gas phases in the urban atmosphere has been studied by filtration and parallel adsorption on active charcoal and polyurethane foam (PUF). Gas chromatography (GC) and GC coupled to mass spectrometry (GC-MS) have been used for the analysis of the organic matter extracts obtained with each system. In the case of the particle and PUF samples these extracts were fractionated into aliphatic and aromatic compounds. This approach has allowed to identify up to 247 hydrocarbon molecules showing that C0–C5 alkylbenzenes are the major compounds in the charcoal extracts whereas C14–C23 n-alkanes, C0–C4 alkylnaphthalenes, C0–C4 alkylbiphenyls and C3–C5 alkylbenzenes are those predominantly found in the PUF materials. The particles essentially contain C17–C38 n-alkanes and parent polycyclic aromatic hydrocarbons (PAH). These qualitative differences are paralleled by a progressive concentration decrease from the more to the less volatile hydrocarbons. Thus, the total charcoal extracts average 80 g/m³, the PUF compounds represent 4 /m³ and the particle hydrocarbons 0.7 g/m³. These latter airborne materials are essentially composed of petrogenic residues 0.6 g/m³ (aliphatic fraction) whereas the pyrolytic PAH only involve 0.08 g/m³.     

LC Method for the Determination of Multiple Components in a Compound Cold Formulation

An isocratic liquid chromatographic method for determination of acetaminophen (AMP), caffeine (CAF), chlorphenamine maleate (CPM) and guaiacol glyceryl ether (GGE) in a compound cold formulation is described. Separation and quantitation were achieved on a Diamonsil C18 column using a binary mixture of methanol and 1.5% aqueous acetic acid (55: 45, v/v, pH 3.6) as mobile phase delivered at 0.4 mL min^–1. Single wavelength detection was at 220 nm for all four drugs and the run time was < 10 min. The linearity, accuracy and precision of the method were found to be acceptable over the concentration ranges: 16.0–127.8 g mL^–1 for AMP, 6.0–48.2 g mL^–1 for CAF, 5.0–40.0 g mL^–1 for CPM and 10.1–80.6 g mL^–1 for GGE.     

Application of Lanthanide-Sensitised Chemiluminescence to the Determination of Levofloxacin, Moxifloxacin and Trovafloxacin in Tablets

A flow injection method including chemiluminescence detection has been developed and applied to the determination of fluoroquinolones levofloxacin, moxifloxacin and trovafloxacin in tablets. The proposed method is based on the luminescent properties of the system Ce(IV)–sulphite–fluoroquinolone and the addition of a trivalent lanthanide ion as emission-sensitizer. The optimum conditions for chemiluminescence emission were investigated for each fluoroquinolone. The best results were achieved when employing Eu(III) as lanthanide cation for levofloxacin and moxifloxacin, and Tb(III) for trovafloxacin. These fluoroquinolones were determined over the concentration range of 0.5–3.5µgmL^–1, 0.2–3.0µgmL^–1 and 0.008–0.400µgmL^–1, with detection limits of 0.100, 0.035 and 0.008µgmL^–1, respectively. The relative standard deviations were in the range of 1.0–2.5% for all three cases. The method was applied to the determination of three fluoroquinolones in their respective pharmaceutical preparations and compared with an independent UV-spectrophotometric method. The results were satisfactory.     

Determination of Proteins at Nanogram Levels Using the Resonance Light Scattering Technique with a Novel PVAK Nanoparticle

A novel functionalized polyvinyl alcohol keto-derivative nanoparticle (PVAK) has been prepared in a one-step method using oxidation and degradation under ultrasonic irradiation. The nanoparticle is water-soluble, chemically stable, non-toxic and biocompatible. The surface of the nanoparticle is covered with abundant hydroxyl, carbonyl and carboxyl. At pH 3.0, the interactions of PVAK with different proteins can result in obviously enhanced RLS signals at 380nm. Under optimal conditions, the calibration graphs are linear over the range of 0.024.0µgmL^–1 for human serum albumin (HSA), 0.023.5µgmL^–1 for bovine serum albumin (BSA), and 0.053.5µgmL^–1 for human -globulin (-G), respectively. Detection limits were 6.4ngmL^–1 for HSA, 9.2ngmL^–1 for BSA, and 12.5ngmL^–1 for -G, respectively. The method was employed for the determination of total proteins in human serum with satisfactory results.     

Simultaneous Determination of Four Active Components in a Compound Formulation by Liquid Chromatography

Summary A rapid and accurate LC method is described for simultaneous determination of pseudoephedrine hydrochloride (PSE), acetaminophen (AMP), dextromethorphen hydrobromide (DEX), and diphenhydramine hydrochloride (DPH) in a compound formulation. Chromatographic separation of the four drugs was achieved on a Hypersil CN column (150 mm × 4.6 mm, 5 m particle) by use of a mobile phase comprising a mixture of 3 mM ion-pairing solution, 2% aqueous triethylamine solution, and 2 M phosphoric acid, 68:48:88 (v/v), pH 3.0, delivered at 1.0 mL min^–1. Compounds were detected at 215 nm and the run time was less than 10 min. The linearity, accuracy, and precision of the method were found to be acceptable over the concentration ranges 6.1–36.4 g mL^–1 for PSE, 65.0–390.0 g mL^–1 for AMP, 3.1–18.6 g mL^–1 for DEX, and 5.0–30.0 g mL^–1 for DPH.     

High-Performance Liquid Chromatographic Determination of Quinolizidine Alkaloids in Radix Sophora Flavescens Using Tris(2,2′-Bipyridyl)Ruthenium(II) Electrochemiluminescence

Electrogenerated chemiluminescences (ECLs) of quinolizidine alkaloids including matrine (MT), sophocarpine (SC), and sophoridine (SRI) are studied. The light emission is caused by an electro-oxidation reaction between Ru(bpy)₃²⁺ and the tertiary amino group on the alkaloid compounds. A thin-layer flow cell equipped with a glassy carbon disk electrode (22.1mm²) at the potential of ⁺1.30V (vs. Ag/AgCl) was applied for ECL observation. MT, SC and SRI were separated and quantitatively determined within 25min by an ODS-80 Ts reversed-phase column with a mobile phase containing 80mmolL^–1 NaH₂PO₄–K₂HPO₄ buffer+acetonitrile (7:3)+40mmolL^–1 sodium dodecyl sulfate (pH 6.5). The determination limit at an S/N of 3 ranged from 3×10^–9gmL^–1 for MT, 6×10^–9gmL^–1 for SC and 1×10^–9gmL^–1 for SRI. The recoveries are from 92 to 108%, with repeatability ranging from 1.3 to 4.5% (relative standard deviation). The method was successfully applied to the determination of quinolizidine alkaloids in Sophora flavescens samples.     

Flow injection chemiluminescence determination of l-cysteine in amino acid mixture and human urine with the BrO3 −–quinine system

In this paper, a novel flow injection chemiluminescence (CL) determination of l-cysteine is proposed. The method is based on the CL reaction of l-cysteine and KBrO₃ in acidic medium. The CL intensity was greatly enhanced in the presence of quinine. The CL intensity was linear with l-cysteine concentration in the range of 0.2–80 g L^–1, and the detection limit was 0.1 g L^–1 (3). A complete analysis, including sampling and injecting, could be performed in 1 min, giving a throughput of about 60 h^–1. The relative standard deviation was 1.6% for 0.8 g L^–1 l-cysteine (n=11). The proposed method was satisfactorily applied to the determination of cysteine in an amino acid mixture and human urine. The mechanism of the CL reaction is also discussed.     

Stereospecific coordination ofl-hydroxyproline esters with triosmium clusters

The reactions of cluster (-H)Os₃(CO)₁₀(-OH) with ethyl and isopropyl esters ofl-oxyproline were studied. In the presence of Me₃NO intermediate complex (-H)Os₃(CO)₉(-OH)L (L — isopropyl ester ofl-oxyproline) is formed, which slowly converts to the more stable cluster (-H)Os₃(CO)₉ . Cluster complexes containing chelate-bridging heterocycles were also obtained by heating (-H)Os₃(CO)₁₀(-OH) with esters ofl-oxyproline. In both cases, only one of the possible diastereomeric complexes (-H)Os₃(CO)₉ (R = Et, Prⁱ) is formed, which indicates that the reactions are stereospecific. Based on analysis of Dreiding's models, an attempt to determine the absolute configuration of the obtained clusters was made.Translated fromIzvestiya Akademii Nauk. Seriya Khimicheskaya, No. 10, pp. 2021–2025, October, 1995.     

Flow-injection/pervaporation coupling for the determination of sulphide in Kraft liquors

A dynamic manifold has been coupled with a pervaporation module for the determination of sulphide ion in complex matrices such as Kraft liquors. The method is based on ethylene blue formation and features detection limits of 0.68 and 0.42 gmL^-1 of S^2- for injection and continuous introduction of the sample, respectively, with linear ranges of 1–15 and 1–10 gmL^-1. The method is highly selective as the interferences from other sulphur species are avoided in the pervaporation process; thus, it has been applied successfully to the determination of the analyte in white and green bleaching liquors.     

Kinetic Spectrophotometric Determination of Trace Aluminum by Catalytic Activity of Al<Superscript>3+</Superscript> on the Oxidation of Methylene Blue by Hydrogen Peroxide

A novel kinetic spectrophotometry for the determination of trace aluminum is described based on the catalytic activity of Al³⁺ on the redox reaction between methylene blue (MB) and hydrogen peroxide in acetate buffer (pH 3.8). The reaction is monitored spectrophotometrically by measuring the decrease in absorbance of the dye at the maximum absorption wavelength of 670nm. The variables that affected the reaction rate were fully investigated, and the optimum conditions were established. Aluminum can be determined in the range of 0–80ngmL^–1 with a detection limit of 1.0ngmL^–1. The relative standard deviation for 10 replicate determinations of 40ngmL^–1 aluminum is 0.9%. The method was used to determine aluminum in tap water and biological samples and produced satisfactory results.Received December 18, 2002; accepted May 5, 2003 published online August 22, 2003     

2,3-Dihydroxypyridine Loaded Amberlite XAD-2 (AXAD-2-DHP): Preparation, Sorption–Desorption Equilibria with Metal Ions, and Applications in Quantitative Metal Ion Enrichment from Water, Milk and Vitamin Samples

2,3-Dihydroxypyridine loaded (via –N=N–linker) Amberlite XAD-2 (AXAD-2-DHP) was prepared and characterized by elemental analyses, TGA and FT-IR spectra. It (1g packed in a column of 1cm diameter; surface area 135.5m²g^–1) was found to be an effective solid phase sorbent for enriching Zn²⁺, Mn²⁺, Ni²⁺, Pb²⁺, Cd²⁺, Cu²⁺, Fe³⁺ and Co²⁺ at pH 3.5 to 7.0 using flow rates between 1.0–5.0mLmin^–1. For desorption (recovery 97.0–99.8%) of the metal ions, 8 to 10mL of 2.0molL^–1 HCl or 1.5molL^–1 HNO₃ at a flow rate of between 2.0 and 4.0mLmin^–1 were found most suitable. The t_1/2 (time for 50% sorption) is between 2 and 10min when a 50mL solution (containing a total amount of metal of 2mg) was equilibrated with 0.5g of resin. Sorption of all metal ions except Pb²⁺ follows the Langmuir model, whereas for Pb the data fits with the Freundlich model. The sorption capacity is between 60.7 (for Cd) and 406.7 (for Cu) µmolg^–1. The resin can withstand an acid concentration of 6molL^–1 and can be reused for thirty cycles of sorption–desorption. The preconcentration factor varies between 100 and 300. For Cd, Ni and Cu the sorption capacity of 2,3-dihydroxypyridine loaded cellulose is lower than that of the present resin. The tolerance limits of electrolytes, humic acid, complexing agents, Ca²⁺ and Mg²⁺ in the enrichment of all metal ions are reported. The limits of detection are 3.88, 5.37, 8.72, 13.88, 4.71, 1.24, 0.59 and 0.30µgL^–1 for Zn²⁺, Mn²⁺, Ni²⁺, Pb²⁺, Cd²⁺, Cu²⁺, Fe³⁺ and Co²⁺, respectively. The calibration curves for flame AAS determination were linear in the ranges 0.018–1.0, 0.067–5.0, 0.2–5.0, 0.9–20, 0.028–2.0, 0.077–5.0, 0.19–10 and 0.1–3.5µgmL^–1, respectively. All the eight metal ions in river and synthetic water samples, Co in vitamin tablets and Zn in milk samples have been quantitatively enriched with Amberlite XAD-2-DHP and determined by flame atomic absorption spectrometry.     

The Fluorescent Reaction Between Quinaldine Red and Nucleic Acids and its Application to Fluorescent Assay of DNA and RNA

The reaction between quinaldine red (QR) and nucleic acids was studied. The free QR alone has no fluorescence in solution. However, it becomes fluorescent after binding to nucleic acids, giving maximum emission at 607nm with maximum excitation at 557nm. Maximum fluorescence intensity is produced in the pH range of 3.2–3.6. Based on the fluorescent reactions, a novel fluorometric method was developed for rapid determination of nucleic acids using QR as the fluorescent probe. Under optimal conditions, the calibration graphs were linear in the range of 0–30.0µgmL^–1 for CT DNA and 0–20.0µgmL^–1 for yeast RNA. The limits of detection were 38ngmL^–1 for CT DNA and 142ngmL^–1 for yeast RNA. Four synthetic samples were determined with satisfaction.Received December 20, 2002; accepted March 27, 2003 Published online August 8, 2003     

Liquid Chromatographic Determination of Sulfamonomethoxine, Sulfadimethoxine, and their N 4-Acetyl Metabolites in Chicken Plasma

An environmentally-friendly method has been established for simultaneous determination of sulfamonomethoxine, sulfadimethoxine, and their N⁴-acetyl metabolites in chicken plasma. The sample is prepared by mixing with 4 mol L^–1 ammonium sulfate solution then centrifugation, and analysis is performed by high-performance liquid chromatography (HPLC) on a polyethylene glycol reversed-phase column with 0.001 mol L^–1 sodium acetate solution as mobile phase and photodiode-array detection. Average recoveries from samples spiked with 0.1, 0.5, and 1.0 g mL^–1 of each drug were >78% and relative standard deviations were within 4%. The practical quantitation limits were 0.09 g mL^–1. No organic solvents or hazardous reagents were used at any stage of the analysis.