Development of an FI-ICP Method for On-Line Preconcentration and Determination of Platinum

This paper presents a new simple and rapid procedure for the preconcentration and determination of platinum. It is based on the adsorption of the metal ion and preconcentration on a micro-column (3cm×3mm) placed in the injection valve of a flow injection (FI) manifold and packed with 1,5-bis[(2-pyridyl)-3-sulphophenyl-methylene]thiocarbonohydrazide (PSTH) immobilised on an anion-exchange resin (Dowex 1X8-200). The metal was eluted from the column using a solution of 2M HNO₃. Various parameters and chemical variables affecting the preconcentration and determination of this metal by ICP-AES were evaluated. Five variables (sample flow rate, eluent flow rate, nebulizer flow rate, buffer concentration and mixing coil length) were considered as factors in the optimisation process. Interactions between analytical factors, and their optimal levels were investigated using two level factorial and central matrix designs. The optimum conditions established were applied to the determination of platinum by flow injection inductively coupled plasma atomic emission spectrometry (FI-ICP-AES). The method has a linear calibration range of 25 to at least 200ngmL^–1 with a detection limit of 7.4ngmL^–1 (S/N=3) and a throughput of 10 samples h^–1 using 5min. preconcentration time. The precision of the method (RSD) was 3.06% ngmL^–1 at the 50ngmL^–1 level of Pt(IV) and 2.93% at the 150ngmL^–1 level. The accuracy of the method was examined by determining the analyte content in spiked waters and by analysing an automobile catalyst standard reference material. The results show good agreement with the certified value and sufficiently high recoveries.     

Determination of Volatile Sulfur Compounds in Beverage and Coffee Samples by Purge-and-Trap On-Line Coupling with a Gas Chromatography-Flame Photometric Detector

A sensitive and fast analytical method using purge-and-trap on-line coupling with gas chromatography was developed for the determination of trace volatile sulfur compounds including dimethyl sulfide (DMS), ethyl-methyl sulfide (EMS), and dimethyl disulfide (DMDS) in beverage and coffee samples. The analytes were purged for 12min from the sample by high purity nitrogen at a flow rate of 35KPa and preconcentrated in the cooled fused-silica capillary trap at –75°C. The NaCl content in the samples was maintained at 10%. The volatile sulfur compounds were separated with an Agilent-6890 gas chromatograph by a suitable temperature program and detected by means of a flame photometric detector (FPD). The detection limits were 80ngL^–1 for DMS, 80ngL^–1 for EMS, and 100ngL^–1 for DMDS, respectively. This method was successfully applied to the determination of volatile sulfur compounds in different beverage and coffee samples.     

Application of Functionalized Ag Nanoparticles for the Determination of Proteins at Nanogram Levels Using the Resonance Light Scattering Method

A novel method for the determination of proteins in aqueous solutions has been developed based on the enhancement of resonance light scattering (RLS) of Ag nanoparticles in the presence of proteins. Factors including acidity of the media, concentration of Ag hydrosol, reaction time, temperature, and interference of non-protein substances were investigated. Under the optimal conditions, with the enhanced RLS signals at 452nm, the linear ranges of calibration curves were 0–0.8µgmL^–1 for bovine serum albumin (BSA), 0–1.2µgmL^–1 for human serum albumin (HSA), and 0–2.5µgmL^–1 for human -IgG (-IgG), respectively. The detection limits were 1.3ngmL^–1 for BSA, 10ngmL^–1 for HAS, and 5.7ngmL^–1 for -IgG.This method has been applied to the analysis of synthetic samples and real human serum samples, and the results were in good agreement with those reported by the hospital, indicating that the method presented here is not only sensitive and simple, but also reliable and suitable for practical applications.     

Determination of Nucleic Acids Based on their Resonance Light Scattering Enhancement Effect on Metalloporphyrin Derivatives

A new method for the determination of nucleic acids at nanogram per mL level is proposed based on the enhanced resonance light scattering (RLS) signal resulting from the interaction of metalloporphyrins with nucleic acids. Under optimum conditions, the weak RLS signal of metalloporphyrin is enhanced by nucleic acids, and the enhanced RLS intensity is proportional to the concentration of nucleic acids. The detection limits of calf thymus DNA were 3.5ngmL^–1, 2.9ngmL^–1 and 1.0ngmL^–1 for three metalloporphyrins, respectively. Synthetic samples were determined with satisfactory results.     

Indirect Determination of Sulfide by Cold Vapor Atomic Absorption Spectrometry

A method for the determination of sulfide based on its interference with the determination of Hg by cold vapor atomic absorption spectrometry is described. The decrease in mercury absorbance at 253.7nm is proportional to the concentration of sulfide over the range of 10–320ngmL^–1. The limit of detection was found to be 7ngmL^–1 and the relative standard deviation (R.S.D.) for the determination of different concentrations of sulfide was in the range of 1.8–2.2%. This method was applied to the determination of sulfide in whole human blood after gas-phase separation.     

Simple and Rapid Method for Determination of Selenium in Breast Milk by HG-AFS

A digestion procedure using H₂SO₄/HNO₃/H₂O₂ was found to be effective for destruction of human milk samples. In conjunction with a sensitive hydride generation atomic fluorescence spectrometry detection system, it is suitable for determination of selenium in those samples where the available mass of breast milk and the low selenium concentration are limiting factors. Only 1g of milk sample is needed. The procedure is simple, rapid and of low contamination potential since it is performed in the same Teflon tube from weighing to measurement. The digestion of 20 samples is completed in three hours. The detection limit is 0.25±0.04ngg^–1 of a measured solution of sample or 2.5ngg^–1 of milk. The relative uncertainty is 10% (coverage factor of 2.3, 95% probability). Because of these advantages the method is particularly suitable for epidemiological studies. The mean concentration of selenium in 62 samples of human milk from lactating women residing in the North East of Italy was 12±3ngg^–1, which is in the range of reference data.     

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.     

Application of L-Cysteine-Capped ZnS Nanoparticles in the Determination of Nucleic Acids Using the Resonance Light Scattering Method

Nanometer-sized L-cysteine-capped ZnS particles were synthesized by a colloidal aqueous method. The functionalized nanoparticles are water-soluble and suitable for biological applications. In Tris-HCl buffer solution, nucleic acids combine with cysteine-capped nano-ZnS particles by intermolecular forces to form larger nanoparticles. There are two resonance light scattering peaks at 304.5nm and 373.8nm, respectively. The enhanced RLS is related to the concentration of nucleic acids in the range of 0.04 to 1.2µgmL^–1 for calf thymus DNA and 0.2 to 1.0µgmL^–1 for fish sperm DNA. The detection limits (3) are 19ngmL^–1 for calf thymus DNA and 23ngmL^–1 for fish sperm DNA, respectively. Four synthetic samples were analyzed satisfactorily.     

Determination of Nucleic Acids Based on Shifting the Association Equilibrium between a Heptamethine Cyanine Dye and Poly-Lysine

A near-infrared (near-IR) fluorescence recovery method for the determination of nucleic acids is presented. This method employs a two-reagent system composed of anionic heptamethines cyanine (HMC) and polycationic poly-lysine. The fluorescence of HMC, with maximum excitation and emission wavelengths at 778 and 804nm, respectively, was quenched by poly-lysine in proper concentration, but recovered by adding nucleic acids. Under optimal conditions, the recovered fluorescence was proportional to the concentration of nucleic acids. The calibration graphs are linear over the range of 5–300ngmL^–1 for herring sperm DNA (FS DNA), 2–100ngmL^–1 for calf thymus DNA (CT DNA) and 5–500ngmL^–1 for snake ovum RNA (SO RNA). The corresponding detection limits are 1.49ngmL^–1 for FS DNA, 0.7ngmL^–1 for CT DNA and 1.61ngmL^–1 for SO RNA, respectively. Four synthetic and three real nucleic acid samples were determined with satisfactory results.     

Determination of Na,K, Rb and Cs Distribution in Human Brain Using Neutron Activation Analysis

This study aims to investigate the distribution of Na, K, Rb and Cs in human brains (5 individuals, 12 brain parts, mean age: 75 years). Distribution of the trace metals between lipid fraction and brain tissue was investigated in solvent extraction experiments. Determinations were carried out by instrumental neutron activation analysis. The present results show a rather non-homogeneous distribution for Na and a relatively uniform distribution for K, Rb and Cs. The mean concentrations found are 7440µgNag^–1 dry weight, 12800µgKg^–1, 14µgRbg^–1 and 50ngCsg^–1. A highly significant positive correlation was found between Rb and Cs. Solvent extraction experiments showed that 19% of Rb and 26% of Cs of the total content is located in lipid fraction.     

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     

Investigation of Medium Power Radiofrequency Capacitively Coupled Plasmas and Their Application to Atomic Emission Spectrometry for the Determination of Aluminium in Water Samples

A medium power radiofrequency capacitively coupled plasma (275W, 27.12MHz) with low argon consumption (0.5Lmin^–1) was investigated to be used for the determination of aluminium in water samples pneumatically nebulised by atomic emission spectrometry. The plasma torch was operated in two geometric configurations, coaxial and coaxial-annular with single (SRTr.f.CCP) or double ring electrodes (DRTr.f.CCP), respectively. The optimum experimental parameters (observation height, Ar flow rate, distance between ring electrodes, matrix interference of Na⁺ and Ca²⁺ and anion nature) for Al 396.152nm emission were established. Under optimum operating conditions of the DRTr.f.CCP torch (6cm distance between annular electrodes), a detection limit of 70ngmL^–1 aluminium was found. Both operating parameters and several figures of merit of the investigated plasmas were compared to those of microwave plasmas and inductively coupled plasma used in atomic emission spectrometry. The method was used to control the quality of drinking and industrial water. Samples were mineralised with 2mL of 1+1 HNO₃ and 10mL of 1+1 HCl. In the range of 0.15–3.5mgL^–1 Al³⁺ the relative standard deviation varied between 3.7 and 8.6% (n=3). For two certified drinking water samples containing 0.206 and 0.218mgL^–1 Al³⁺ the recovery (n=5) was 97.6±6.8% and 98.6±7.3%, respectively.     

Determination of cadmium and bismuth in high-purity zinc metal by inductively coupled plasma mass spectrometry with on-line matrix separation

Traces of cadmium and bismuth in high-purity zinc metal were determined by inductively coupled plasma mass spectrometry (ICP-MS) in combination with flow injection (FI) on-line matrix separation (FI-ICP-MS). The anion-exchange separation method of the potassium iodide (KI) system was applied to the separation of the analytes from the matrix zinc. The analytes, cadmium and bismuth, were adsorbed on the anion-exchange (BIORAD AG1-X8) mini-column (1.0 mm i.d.× 100 mm bed length), while the matrix zinc can be completely removed from the anion-exchange resin. The analytes were eluted by 2 mol/l HNO₃ and directly introduced into the ICP-MS. The detection limits (D.L.) obtained by using a single injection (350 l) were 0.81 and 0.075 ngg^-1 for cadmium and bismuth, respectively. In the case of multi-injection concentration onto the anion-exchange mini-column (five injections 350 l each), the detection limits could be improved to 0.16 and 0.014 ngg^-1 for cadmium and bismuth, respectively. The reproducibilities of the single injection and the multi-injection method were satisfactory with a relative standard deviation of less than 5% (at the 10 and 1 ngml^-1 level for the single injection and the multi-injection method, respectively). The method was successfully applied to the determination of trace impurities in four samples of high-purity zinc metal (7 nines grade) and three standard reference materials of high-purity unalloyed zinc samples (from NIST).     

Determination of Picogram-Levels of Acetylspiramycin in Human Urine and Serum by Flow Injection Chemiluminescence

A sensitive chemiluminescence method for the determination of acetylspiramycin is presented. It is based on the greatly enhancive effect of acetylspiramycin on the chemiluminescence reaction between luminol and hydrogen peroxide in the flow system. The increase in chemiluminescence intensity was linearly proportional to the acetylspiramycin concentration in the range from 10pg·mL^–1 to 2.0ng·mL^–1 (r²=0.9979). The detection limit was 3pg·mL^–1 (3). At a flow rate of 2.0mL·min^–1, the process of determination, including sampling and washing, could be performed in 0.5 min, and the relative standard deviations of seven replicates are less than 5.0%. The proposed method was applied successfully to the determination of acetylspiramycin in pharmaceutical preparations, human urine and serum without pre-treatment. It was found that the excretive ratio of acetylspiramycin reached its maximum 2.0 hours after having been administered orally, and the excretive ratio in 12.0 hours was 8.4.     

Determination of Trace Proteins by Rayleigh Light Scattering Technique with Indophenol Blue

The interaction of indophenol blue (IPB) with proteins in aqueous solution has been studied by optical absorption and Rayleigh light scattering (RLS) spectroscopy. At pH 3.8, the weak RLS of IPB is enhanced by proteins. Based on this phenomenon, a novel method for the determination of proteins at nanogram levels using the RLS technique is developed. The method is simple, practical and sensitive. The linear range is 0.25–20.9µgmL^–1 for BSA, and 0.25–17.6µgmL^–1 for HSA. The detection limits (S/N=3) are 23ngmL^–1 for BSA and 22ngmL^–1 for HAS. The results for the determination of proteins in human serum samples are very close to those obtained by an established clinical method. There is very little interference from amino acids, metal ions or other coexisting compounds.     

Determination of the Antibacterial Drug Enrofloxacin by Solid-Phase Spectrofluorimetry

A method for the determination of trace amounts of enrofloxacin based on solid-phase spectrofluorimetry has been developed. The relative fluorescence intensity of enrofloxacin fixed on Sephadex SP C-25 gel was measured directly after packing the gel beads in a 1-mm silica cell, using a solid-phase attachment. The wavelengths of excitation and emission were 277 and 448nm, respectively. The linear concentration range of application was 0.2–4.0ngmL^–1 of enrofloxacin, with a relative standard deviation of 1.2% (for a level of 2.0ngmL^–1) and a detection limit of 0.04ngmL^–1. The method was applied to the determination of enrofloxacin in commercial pharmaceutical formulations and spiked canine serum samples. It was validated using HPLC as a reference method and applying the standard addition methodology. Recovery levels of the method reached 100% in all cases.     

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.     

Non-Aqueous Capillary Electrophoresis with Indirect Photometric Detection for Direct Analysis of Pb2+, Zn2+ and Cd2+ Ions

A new approach, based on non-aqueous capillary electrophoresis separation and indirect photometric detection, was established for the determination of the transition metal ions Pb²⁺, Zn²⁺ and Cd²⁺. Under optimized conditions, the method produced baseline separation of these three metal ions. The linear range and detection limits were 1050µM, 1.9µM for Cd²⁺; 1050µM, 2.1µM for Zn²⁺; and 20100µM, 3.8µM for Pb²⁺, respectively.     

Kinetic Spectrophotometric Determination of Total Iron in Natural Water by Flow Injection Analysis Using On-Line Preconcentration

A new flow injection catalytic spectrophotometric method for on-line preconcentration and determination of total iron in natural water is described. The method is based on a combination of iron-catalyzed oxidation of diaminoditolyl by potassium bromate and the use of on-line preconcentration of iron onto 8-hydroxy-quinoline immobilized on silica gel. The corresponding calibration graph is linear over the range of 2.0–110ngmL^–1 for Fe(III) using a time-based technique for 5min preconcentration. The relative standard deviation of 11 measurements of 60ngmL^–1 Fe(III) was 0.67%. The method was applied to the determination of iron in natural water. The results obtained by the proposed method were compared with those obtained by ICP-AES. The t-test showed no significant differences between the two methods at a confidence level of 95%.     

Determination of Heavy Metal Ions in Chinese Herbal Medicine by Microwave Digestion and RP-HPLC with UV-Vis Detection

A new method for the simultaneous determination of heavy metal ions in Chinese herbal medicine by microwave digestion and reversed-phase high-performance liquid chromatography (RP-HPLC) has been developed. The Chinese herbal medicine samples were digested by microwave digestion. Lead, cadmium, mercury, nickel, copper, zinc, and tin ions in the digested samples were pre-column derivatized with tetra-(4-chlorophenyl)-porphyrin (T₄-CPP) to form the colored chelates which were then enriched by solid phase extraction with C₁₈ cartridge and eluted from the cartridge with tetrahydrofuran (THF). The chelates were separated on a Waters Xterra RP₁₈ column by gradient elution with methanol (containing 0.05molL^–1 pyrrolidine-acetic acid buffer salt, pH=10.0) and THF (containing 0.05molL^–1 pyrrolidine-acetic acid buffer salt, pH=10.0) as mobile phase at a flow rate of 0.5mLmin^–1 and detected with a photodiode array detector in the range of 350–600nm. In the original samples the detection limits of lead, cadmium, mercury, nickel, copper, zinc and tin are 4ngL^–1, 3ngL^–1, 6ngL^–1, 5ngL^–1, 2ngL^–1, 6ngL^–1, and 4ngL^–1, respectively. This method was applied to the determination of lead, cadmium, mercury, nickel, copper, zinc and tin in Chinese herbal medicine samples with good results.