Determination of thiamine using continuous flow molecular emission cavity analysis

A continuous flow method for the determination of thiamine hydrochloride (20.0-240.0 microgram ml(-1), 5.9 x 10(-5)-7.1 x 10(-4)m) is described. The sample was mixed with an excess of sodium hydroxide and remained in the delay coil for 20 min at 90 degrees C. The solution was then mixed with an excess of orthophosphoric acid and the hydrogen sulphide evolved was transferred continuously into the cavity to generate a molecular++ emission of S2. The analysis is completely automated, requires no sample pre-treatment and samples can be analysed at a rate of 30 samples h(-1) with a relative error of 1-2%. The method was evaluated by carrying out an interference study with common excipients and other water-soluble vitamins, a recovery study and by the analysis of commercial formulations. Results compared well with those obtained using the official method. The method was also applied to content uniformity tests.     

Improved scheme of chelation ion chromatography with a mixed eluent for the simultaneous analysis of transition metals at microg l(-1) levels

An improved scheme of chelation ion chromatography (CIC) system and a mixed eluent for the simultaneous determination of transition metals are described. A method based on the improved CIC system and the mixed eluent (PDCA/Na2C2O4/LiOH/NaCl) for the analysis of seven metals (Pb2+, Cu2+, Ni2+, Zn2+, Co2+, Cd2+ and Mn2+) at microg l(-1) levels in a single isocratic elution is developed. The optimize conditions which are different from references for analyte concentration and chromatographic separation are studied in detail. D418 chelation resin is used to further reduce values of the reagent blank. The above seven metals are measured at 565 nm using 2-[(5-Bromo-2-Pyridyl)-Azo]-5-Diethyl-AminoPhenol(5-Br-PADAP) as the post-column derivatizing reagent. Detection limits range from 0.3 to 12 microg l(-1) when 4 ml of sample is pre-concentrated. The results of real sample analysis are satisfactory.     

On-line column preconcentration for the determination of cobalt in sea water by flow-injection chemiluminescence detection

A flow-injection method for the determination of dissolved cobalt(II) in sea water has been studied based on a combination of column preconcentration using 8-quinolinol immobilized on silica gel, fluoride containing metal alkoxide glass (8HQ-MAF) and chemiluminescence detection with a gallic acid-hydrogen peroxide system. Co(II) is selectively recovered from an acidified sample with 8-quinolinol immobilized on silica gel. After elution with dilute hydrochloric acid the resultant eluent is mixed with the reagent solutions, heated to 60 ( degrees )C and then introduced into the CL cell. The analysis time including the 2-min sample load was 8 min per sea water sample with a corresponding detection limit of 0.62 ng l(-1) (3sigma). The average standard deviation calculated for 10 replicate measurements of artificial sea water samples with a concentration of 10 ng l(-1) cobalt was +/-2.1%. The method has been tested with the standard reference sea waters NASS and CASS.     

外标归一化气相法测定天然气组成

 对SP 6000天然气分析仪的气路系统作了改进,实现了仪器自身标定。采用填充柱和毛细管柱分离,热导检测器和火焰电离检测器双检测器检测,外标 归一化法定量,简易、快速地测定了天然气组成。方法的准确度及精密度均符合气相法定量分析的要求。     

核级碳化硼试样分解方法的研究

在对核级碳化硼试样的多种分解方法进行简要介绍和分析之后,提出了以碳酸钙作熔剂在高温下分解试样,以盐酸浸取的方法,此方法应用于核级碳化硼中总硼、铁、铝等的测定获得了满意的结果。     

Modification of AOAC method 973.31 for determination of nitrite in cured meats

A modification of AOAC Method 973.31 is proposed to improve the extraction efficiency of nitrite from cured meat samples and its subsequent quantification based on the diazotization-coupling reaction of sulfanilamide with N-(1-naphthyl)ethylenediamine dihydrochloride (NED). The various experimental parameters were thoroughly investigated. A 5 g meat sample was mixed with 400 mL water; the pH of the mixture was adjusted to 5.5 +/- 0.3 and allowed to stand for 2 h on a water bath at 80 degrees C, with occasional shaking for the complete extraction of nitrite. After quantitative filtration, an aliquot was mixed with chloroacetic-chloroacetate buffer, pH 1.80 +/- 0.05, sulfanilamide, and NED, and the absorbance of the resulting azodye was recorded at 540 nm against water as a reference. Following the recommended procedure, a linear calibration graph was obtained for up to 0.8 microg/mL NO2(-), with a correlation coefficient of 0.9996 and a detection limit (based on the 3 Sb-criterion) of 5.6 ng/mL NO2(-). The proposed method was conveniently applied to various cured meat samples and was validated by comparison with the original AOAC method and by recovery experiments that gave quantitative results (94-98%) with convenient reproducibility. Statistical analysis of the analytical data could not detect any systematic error and revealed the high accuracy and precision of the proposed method.     

Rapid determination of sulphonamides in milk using liquid chromatographic separation and fluorescamine derivatization.

A simple and selective method is presented for the multiple residue determination of eight sulphonamides in consumers' milk. The drugs are sulphisomidine (ID), sulphadiazine (DZ), sulphamerazine, sulphadimidine, sulphamonomethoxine, sulphamethoxazole, sulphadimethoxine and sulphaquinoxaline (SQ). The milk sample was deproteinized with the same volume of 2 M hydrochloric acid and filtered. A 1-ml volume of the filtrate was mixed with 1 ml each of 1.25 M sodium acetate solution and a buffer (pH 3.0) for derivatization with 0.6 ml of 0.02% fluorescamine solution in acetone. A high-performance liquid chromatographic analysis was carried out on a C18 column with a mobile phase of acetonitrile-2% acetic acid (3:5) at 55 degrees C using a fluorescence detector at an excitation wavelength of 405 nm and an emission wavelength of 495 nm. Average recoveries at fortification levels of 2, 5 and 10 ng/ml were 114%, 109% and 106%, respectively. Relative standard deviations were 1-4% at 10 ng/ml for ID, 5 ng/ml for DZ and SQ and 2.5 ng/ml for the other five sulphonamides. The method was applied to 25 milk samples and all appeared to be free from the drugs.     

Precolumn derivatization liquid chromatography method for analysis of dietary supplements for glucosamine: single laboratory validation study

A precolumn derivatization liquid chromatography (LC) method was developed for the analysis of various dietary supplement formulations and raw materials for glucosamine. A 1 mL sample or standard water solution (containing about 0.05 mg glucosamine) was mixed with 1 mL pH 8.3 buffer, 1 mL 5% phenylisothiocyanate methanolic solution, and derivatized at 80 degrees C in a water bath for 30 min. After derivatization, the solution was cooled in a cold water bath and centrifuged at 3000-5000 rpm. The clear upper layer was ready for injection. The LC system was equipped with a C18 reversed-phase column and an ultraviolet detector set at 240 nm. The column was developed with a linear gradient composed of 0.1% phosphoric acid in deionized water and 0.1% phosphoric acid in methanol. The method was subjected to Single Laboratory Validation. The method precision was 0.50% relative standard deviation, accuracy was less than +/-1.5%, method linearity in the range 0-2 mg glucosamine/mL was 1.00, the detection limit was 0.0705 microg/mL, and the quantitation limit was 0.235 microg/mL. Chondroitin sulfate, amino acids, and excipients did not interfere with glucosamine testing. After derivatization, both standard and sample preparations were stable for at least 48 h. Due to its high sensitivity, this method can be used to assay glucosamine in functional foods and pet foods. The validation data will be published separately.     

Application of matrix solid-phase dispersion in the determination of dibenzo[a,l]pyrene content of experimental animal diets used in a large-scale tumor study.

A method utilizing matrix solid-phase dispersion (MSPD) was developed for isolation and determination of dibenzo[a,l]pyrene (DBP) in experimental rainbow-trout diets used in a large-scale carcinogenesis study. A 0.5 g sample of moist ration containing 0-225 ppm DBP (dry basis) was mixed with 2 g C18 sorbent and benzo[a]pyrene internal standard was added to the mixture. Extraction and clean-up were accomplished in a single step by extracting the sample mixture with hexane-benzene 4:1 from a cartridge containing 2 g Florisil. DBP was quantified by HPLC on a C5 bonded phase column with fluorescence detection. Mean analytical recovery of DBP from control diet spiked at three concentration levels was 101 to 107% with relative standard deviations of 1 to 7%. The limit of detection of DBP was equivalent to 0.014 ppm in the ration. Application of the method to verification of DBP levels in trout rations from the carcinogenesis study is described. Control ration (0 ppm DBP) was screened for possible DBP contamination and none was found. This is the first report on analysis of DBP in experimental animal diets.     

Comparison of potentiometric titration,IR spectrophotometry and segmented micro-flow analysis to determine inorganic C in alkaline solutions

A segmented micro-flow analysis procedure was described for the determination of total carbonates in alkaline solutions. The method is based on CO(2) diffusion from an acidified sample through a silicone membrane. The gas is then collected in a coloured acceptor solution. The decolouration of the solution due to the trapped CO(2) is then determined by spectrophotometry at a wavelength of 550 nm. The method was evaluated for the range 0-1000 mg C CO(2) L(-1) at a sampling frequency of 60 h(-1). The method was repeatable (RSD better than 1%), accurate (1.5 and 2.5% for standards) and the limit of detection was close to 6 mg C CO(2) L(-1). The results were also compared with those obtained by the potentiometric reference method (PT) and an infrared spectrometric method (IRS). The measurements obtained showed good agreement with those obtained using PT and IRS methods, the PT method being the most accurate. The SFA method appeared to be a really efficient and a more suitable technique for routine C CO(2) determination, although some results showed that for standard solutions, the measured concentrations were significantly different from those obtained with the PT method for concentrations higher than or equal to 800 mg C CO(2) L(-1). For 0.25 M NaOH samples, the three methods tested gave similar results in the range 0-600 mg C CO(2) L(-1).     

Estimation of cyclosporin-A in whole blood by simple and rapid reversed-phase HPLC utilizing a salting-out extraction procedure

Cyclosporin-A is a fungal cyclic undecapeptide immunosuppressive agent that is potentially active against proliferating T-lymphocytes and therefore helps the body to accept a transplanted organ. In this experiment, the drug is extracted from whole blood with acetonitrile. The extraction solvent (acetonitrile) is mixed with the whole blood at a 1:2 ratio on a vortex mixer and is centrifuged at 2000 x g. The supernatant is transferred into a fresh borosilicate culture test tube and 20 mg of zinc sulfate and 10 mg of cadmium sulfate (for 1.0 mL of whole blood) are added, vortex mixed, and centrifuged at 2000 x g. The supernatant is saturated with anhydrous ammonium sulfate and centrifuged, and salted-out acetonitrile from the aqueous mixture is injected into the HPLC system. A 60- x 4.6-mm 3-microns, slurry-packed ODS (C18) column is used with an isocratic elution of 66:2:32 (v/v), acetonitrile-isopropanol-water. The column temperature is maintained at 72 degrees C. Cyclosporin-A is detected by UV absorption at 205 nm and 0.10 to 0.002 AUFS. The limit of detection of the method is 15 ng/mL for a 100-microL injection volume, and the completion time for analysis of one sample is less than 15 min. Columns packed with different stationary phases and different dimensions are investigated to determine which column will give the maximum resolution, sensitivity, and selectivity.     

Automated high-performance liquid chromatographic determination of 5-S-cysteinyl-3,4-dihydroxyphenylalanine in urine

An automated high-performance liquid chromatographic (HPLC) method has been developed for measurement of 5-S-cysteinyl-DOPA in urine (DOPA = 3,4-dihydroxyphenylalanine). The urinary sample was injected into an HPLC boronate column. With a mobile phase of 0.1 M phosphate buffer containing 0.2 mM disodium ethylenediaminetetraacetate (Na2EDTA) (pH 6.0) mixed with methanol (9:1), 5-S-cysteinyl-DOPA was adsorbed while most other compounds were washed away. By column switching, the column flow was reversed and 5-S-cysteinyl-DOPA was desorbed by a mobile phase of 0.1 M formic acid and 0.2 mM Na2EDTA at pH 3.0 and chromatographed on a reversed-phase column. The precision, as estimated from repeated analysis of an urinary sample and from duplicate analysis of a number of samples, ranged from 1.4 to 5.2% (coefficient of variation), and the analytical recovery was 93 +/- 4.1%. The method is suitable for use in the clinical laboratory.     

Fluorimetric determination of alkaline phosphatase in solid and fluid dairy products

A new assay has been developed for measuring residual alkaline phosphatase (ALP) activity in a wide variety of dairy products. The method proposed is simple, rapid and directly applicable to solid and liquid dairy samples. ALP in the test sample hydrolyzes a non fluorescent substrate, trifluoromethyl-β-umbelliferone phosphate, to its highly fluorescent phenolate product. The assay is performed in a reverse micellar medium composed of mixed buffer (2-amino-2-methyl-1-propanol buffer pH 9.0 and borate buffer pH 9.0) in AOT/isooctane, at a temperature of 38 °C. Total test time is 450 s. Reaction rates are linear (except for butter) up to 8.5 and 11% (v/v) raw milk, for whole milk and chocolate milk, respectively. The detection limits are 0.04, 0.4 and 0.22% (v/v) raw milk, for whole milk, chocolate milk and butter, respectively. The precision of the fluorimetric method was assessed by repeated analysis of a pasteurized milk sample spiked with mixed herd raw milk. The accuracy of the method was evaluated by comparison with an official colorimetric assay using p-nitrophenylphosphate as ALP substrate.     

Open tube combustion method of organic samples for stable carbon isotope analysis

A simple and effective method for the conversion of organic carbon into carbon dioxide for analysis of stable carbon isotopes (delta(13)C) in samples of various organic substances, soils, sedimentary rocks, oils and volatile organic liquids is presented. The conversion of organic carbon of the samples is carried out in a quartz reactor connected to a vacuum line for CO(2) freezing and purification. A solid organic sample mixed with CuO is placed at the reactor bottom and the reactor is subsequently filled with granular CuO. One end of the CuO column is preheated to 850 degrees C while the other end of the column in contact with the sample is kept at ambient temperature. Heating of the sample (850 degrees C) and the remainder of the column is then performed. The preheated part of the column provides efficient conversion of carbon into CO(2). The reactor for the conversion of volatile liquid organic compounds is filled with granular CuO. The column of CuO is heated to 850 degrees C. Samples of volatile liquids are introduced into the reactor through a septum using a microsyringe. Complete conversion takes 10 min for solid samples and 3 min for volatile liquids. The precision of the delta(13)C analysis for solid and volatile liquid organic substances is +/-0.1 per thousand and +/-0.04 per thousand, respectively.     

傅里叶变换红外光声光谱法在聚合物研究中应用——Ⅱ.定量测定组合浆料中变性聚乙烯醇

本文叙述了用傅里叶交换红外光声光谱法测定组合浆料中变性聚乙烯醇和淀粉醋酸酯混合比的快速定量分析方法。变性聚乙烯醇和淀粉醋酸酯的红外光声光谱和红外吸收光谱具有相同图谱。观察了干涉仪动镜扫描速度,扫描次数及试样用量对红外光声光谱信号强度的影响。以变性聚乙烯醇的C=O伸缩振动1570cm~(-1)作为定量分析依据。变性聚乙烯醇含量与1600～1516cm~(-1)范围内的积分强度值成线性关系。用红外光声光谱法测定混合试样中变性聚乙烯醇含量与真实值相吻合。     

氢氧化锰共沉淀分离-催化极谱法测定土壤中有效钼

土壤样品中有效钼用草酸铵-草酸混合溶液(pH 3.3)振摇提取,所得悬浮液用干滤纸过滤,分取部分滤液蒸缩体积后加入10 g.L-1酸性高锰酸钾溶液并蒸发至近干,趁热加0.25 mol.L-1氢氧化钠溶液进行共沉淀分离。分取部分上清液,用硫酸(1+1)溶液酸化后加入混合底液(其中含有二苯基乙醇酸、二苯胍及氯酸钠)及少许钛铁试剂溶液作为与钼(Ⅵ)进行催化反应的试剂体系。用JP-303极谱仪进行测定。在-220 mV峰电位处测得的峰电流值与其相应的钼(Ⅵ)的质量浓度在0.8～20μg.L-1范围内呈线性关系。此方法的检出限(3s/k)为0.002 6μg.g-1。用此方法分析了5个土壤标准物质,所测得有效钼的含量与其认定值相符。     

An online method combining a thermal conversion elemental analyzer with isotope ratio mass spectrometry for the determination of hydrogen isotope composition and water concentration in geological samples

An online continuous-flow method, combining a thermal conversion elemental analyzer (TC/EA) with isotope ratio mass spectrometry (MS), is evaluated for the determination of both the hydrogen isotope composition and the water concentration of hydrous and nominally anhydrous minerals. The technique involves reduction of hydrous minerals or nominally anhydrous minerals by reaction with glassy carbon at 1450 degrees C in a helium stream. The product gases, H2 and CO, are separated on a gas chromatographic column prior to analysis in the mass spectrometer. Calibration curves for the H concentration analysis were generated from a standard of benzoic acid (C7H6O2) that has an H concentration of 5.0 wt%; the analytical uncertainties were better than +/-0.05% in our runs. Two standards of material with given D values, polyethylene IAEA-CH-7 and biotite NBS-30, were tested for the purpose of calibrating a natural garnet 04BXL02 representing nominally anhydrous minerals. Preheating at 90 degrees C for 12 h was found to be suitable for removing adsorption water on the sample surface. This results in constant D values and total H2O contents for the garnet, with weighted means of -94 +/- 1 and 522 +/- 11 ppm (wt), respectively. The TC/EA-MS technique allows routine analysis of sample sizes as small as 0.01 microL H2O. For natural minerals, absolute reproducibilities for D values are +/-0.5 to +/-2 (1) and relative uncertainties for total H2O concentrations are at levels of +/-1% to +/-3% (1). Therefore, this online method can be used for the quantitative determination of H isotope composition and H2O concentration of either hydrous or anhydrous minerals.     

Synthesis and Characterization of Indium-borate Glass-ceramics Containing Ho0.01Ce0.74Zr0.25O1.995 Nanorods via Incorporation Method

Glasses in the system 5In₂O₃·94Na₂B₄O₇ were fabricated via melt quenching technique. The amorphous nature of the quenched glasses was confirmed by X‐ray powder diffraction studies, and the infrared spectra of the glasses show no boroxol ring formation in the structure of these glasses. Differential thermal analysis is shown glass transition temperature 696°C and crystallization temperature 1151°C. A cerium‐zirconium mixed oxide Ce_0.75Zr_0.25O₂ and Ho‐doped cerium‐zirconium mixed oxide were obtained by solid‐state method. Then glass powder and Ho‐doped cerium‐zirconium mixed oxide were mixed. The mixture was heated in a crucible. The glass‐ceramic sample was obtained by pouring the melts on stainless steel. Obtained samples were annealed at 450°C for 1 h to remove thermal strain. Differential thermal analysis for glass‐ceramic sample is shown glass transition temperature 668°C and crystallization temperature 1159°C. The scanning electron microscopy study for glass‐ceramic indicates that the crystallized glass consists of rod‐like crystals with average diameter of about 38 nm dispersed in the glassy regions.     

Mobile, outdoor continuous-flow isotope-ratio mass spectrometer system for automated high-frequency 13C- and 18O-CO2 analysis for Keeling plot applications

A continuous-flow isotope-ratio mass spectrometer (CF-IRMS, custom-made GasBenchII and Delta(plus)Advantage, ThermoFinnigan) was installed on a grassland site and interfaced with a closed-path infrared gas analyser (IRGA). The CF-IRMS and IRGA were housed in an air-conditioned travel van. Air was sampled at 1.5 m above the 0.07-m tall grassland canopy, drawn through a 17-m long PTFE tube at a rate of 0.25 L s(-1), and fed to the IRGA and CF-IRMS in series. The IRMS was interfaced with the IRGA via a stainless steel capillary inserted 0.5 m into the sample air outlet tube of the IRGA (forming an open split), a gas-tight pump, and a sample loop attached to the eight-port Valco valve of the continuous-flow interface. Air was pumped through the 0.25-mL sample loop at 10 mL s(-1) (a flushing frequency of 40 Hz). Air samples were analysed at intervals of approx. 2.8 min. Whole system precision was tested in the field using air mixed from pure CO2 and CO2-free air by means of mass flow controllers. The standard deviation of repeated single measurements was 0.21-0.07 per thousand for delta13C and 0.34-0.14 per thousand for delta18O of CO2 in air with mixing ratios ranging between 200-800 micromol mol(-1). The CO2 peak area measured by the IRMS was proportional to the CO2 mixing ratio (r2 = 1.00), allowing estimation of sample air CO2 mixing ratio from IRMS data. A 1-day long measurement cycle of CO2, delta13C and delta18O of air sampled above the grassland canopy was used to test the system for Keeling plot applications. Delta18O exhibited a clear diurnal cycle (4 per thousand range), but short-term (1-h interval) variability was small (average SD 0.38 per thousand). Yet, the correlation between delta18O and CO2 mixing ratio was relatively weak, and this was true for both the whole data set and 1-h subsets. Conversely, the delta13C of all 541 samples measured during the 25.2-h interval fitted well the Keeling regression (r2 = 0.99), yielding an intercept of -27.40 per thousand (+/-0.07 per thousand SE). Useful Keeling regressions (r2 > 0.9, average r2 = 0.96) also resulted from data collected over 1-h intervals of the 12-h long twilight and dark period. These indicated that 13C content of ecosystem respiration was approx. constant near -27.6 per thousand. The precision of the present system is similar to that of current techniques used in ecosystem studies which employ flask sampling and a laboratory-based CF-IRMS. Sampling (and measurement) frequency is greatly increased relative to systems based on flask sampling, and sampling time (0.025 s per sample) is decreased. These features increase the probability for sampling the entire CO2 range which occurs in a given time window. The system obviates sample storage problems, greatly minimises handling needs, and allows extended campaigns of high frequency sampling and analysis with minimal attendance.     

Rapid spectrophotometric determination of total phosphorus in industrial wastewaters by flow injection analysis including a capillary digestor

The method described is suitable for the rapid determination of total phosphorus in industrial wastewaters. A coiled teflon capillary digestor (10 m long, 1 mm i.d.), which contains a platinum wire as catlyst for oxidation with potassium peroxodisulfate at 160°C, is directly connected to the color-development system based on ion-pair formation between molybdophosphate and malachite green. A single determination of total phosphorus can be completed in 4 min. Calibration graphs are linear for ranges of 0–500 and 10–50 ng ml^-1 phosphorus. The determination limit is 2 ng ml^-1 phosphorus when the sample injection volume is optimized for a given analyte concentration. Applications to seawaters and industrial wastewaters mixed with seawater are discussed. Results are in good agreement with those obtained by the standard method.