Simultaneous fluorimetric determination of acetylsalicylic acid metabolites in urine by partial least squares multivariate calibration

A method is described for the simultaneous determination of the main urinary acetylsalicylic acid (aspirin) metabolites, salicyclic, salicyluric and gentisic acids, based on their native fluorescence. The urine was extracted into diethyl ether in acid medium, and back-extracted with glycine/sodium hydroxide buffer solution at pH 9.4. A comparative study of the results found using the excitation, the emission and the combination of the excitation plus the emission spectral data, as analytical signals, was performed. The data set, composed of the excitation plus the emission spectra, was selected as the analytical signal. The optimum wavelengths to record the excitation (lambda(em)=444 nm) and the emission spectra (lambda(ex)=323 nm) were selected to maximize the contribution from gentisic acid, which is the minor urinary metabolite. Partial least squares (PLS-1) multivariate calibration was then applied for the determination. Recovery values from urine samples spiked with salicyclic, salicyluric and gentisic acids varied from 90.1 to 97.6% (mean 93.6%), from 90.0 to 110% (mean 97.9%) and from 89.9 to 104.7% (mean 98.5%), respectively.     

Simultaneous fluorimetric determination of acetylsalicylic acid metabolites in urine by partial least squares multivariate calibration

A method is described for the simultaneous determination of the main urinary acetylsalicylic acid (aspirin) metabolites, salicyclic, salicyluric and gentisic acids, based on their native fluorescence. The urine was extracted into diethyl ether in acid medium, and back-extracted with glycine/sodium hydroxide buffer solution at pH 9.4. A comparative study of the results found using the excitation, the emission and the combination of the excitation plus the emission spectral data, as analytical signals, was performed. The data set, composed of the excitation plus the emission spectra, was selected as the analytical signal. The optimum wavelengths to record the excitation (_em=444 nm) and the emission spectra (_ex=323 nm) were selected to maximize the contribution from gentisic acid, which is the minor urinary metabolite. Partial least squares (PLS-1) multivariate calibration was then applied for the determination. Recovery values from urine samples spiked with salicyclic, salicyluric and gentisic acids varied from 90.1 to 97.6% (mean 93.6%), from 90.0 to 110% (mean 97.9%) and from 89.9 to 104.7% (mean 98.5%), respectively.     

High-performance liquid chromatographic method for the determination of salicylic acid and its metabolites in urine by direct injection

A direct injection method has been developed for the determination of salicylic acid and its metabolites in urine. Urine samples are treated with hydroxylamine to convert salicyl acyl glucuronide to salicylhydroxamic acid, which can be accurately quantitated by direct injection into a high-performance liquid chromatographic system along with salicylic acid, gentisic acid and salicyluric acid. Salicyl phenolic glucuronide is quantitated by difference after hydrochloric acid hydrolysis at 65 degrees C with no loss of salicylic acid by sublimation or hydrolytic loss of salicyluric acid. This method has been applied to urine samples from human subjects and the results are discussed.     

Resolution of ternary mixtures of salicylic, salicyluric and gentisic acids by partial least squares and principal component regression: Optimization of the scanning path in the excitation-emission matrices

The resolution of ternary mixtures of salicylic, salicyluric and gentisic acids has been accomplished by partial least squares (PLS) and principal component regression (PCR) multivariate calibration. The total luminescence information of the compounds has been used to optimize the spectral data set to perform the calibration. A comparison between the predictive ability of the three multivariate calibration methods, PLS-1, PLS-2 and PCR, on three spectral data sets, excitation, emission and synchronous spectra, has been performed. The excitation spectrum has been the best scanning path for salicylic and salicyluric acid determinations, while the emission spectrum has been the best for the gentisic acid determination. The convenience of analysing the total luminescence spectrum information when using multivariate calibration methods on fluorescence data is demonstrated.     

Simultaneous determination of acetylsalicylic acid and its major metabolites in human serum by second-derivative synchronous fluorescence spectrometry.

A method is described for the simultaneous determination of acetylsalicylic, salicylic, gentisic and salicyluric acids (ASA, SA, GA and SU, respectively) in serum, based on their native fluorescence. The ASA-SA-GA-SU-containing serum samples are extracted with chloroform-1% acetic acid solution; ASA and SA are determined in the organic phase, and GA and SU in the aqueous phase, after removal of protein with trichloroacetic acid, at pH 5.0 and 11.6, respectively. The ASA-SA and GA-SU-SA mixtures are resolved using second-derivative fluorescence spectrometry and the appropriate empirical equations involving the effect of each acid on the signal of the other. Recoveries from sera spiked with ASA (1.0-10 micrograms ml-1), SA (25-50 micrograms ml-1), GA (0.05-0.2 micrograms ml-1) and SU (1.0-5.0 micrograms ml-1) ranged from 100 to 104% (mean 101%), from 93 to 99% (mean 97%), from 94 to 104% (mean 99%) and from 94 to 107% (mean 98%), respectively.     

A new spectrophotometric method for quantitative multicomponent analysis resolution of mixtures of salicylic and salicyluric acids

A new spectrophotometric method for resolving binary mixtures is proposed. The method is based on use of the first derivative of the ratios of spectra. The absorption spectrum of the mixture is obtained and the amplitudes at appropriate wavelengths are divided by the corresponding amplitudes in the absorption spectrum of a standard solution of one of the components, and the first derivative of the ratio spectrum is obtained. The concentration of the other component is then determined from a calibration graph. The method has been applied for resolving binary mixtures of salicylic and salicyluric acids. Calibration graphs for 2.6-52 ppm salicylic acid and for 2.1-42 ppm salicyluric acid were established by measuring the analytical signals at the maximum at 241.5 nm (for salicylic acid) and from the peak at 258 nm to the trough at 247 nm (for salicyluric acid) in the first derivative ratio spectra.     

Trilinear PARAFAC decomposition of synchronous fluorescence spectra of mixtures of the major metabolites of acetylsalicylic acid

Mixtures of the three major metabolites of acetylsalicylic acid (salicylic, gentisic and salicyluric acid) were analyzed by synchronous molecular fluorescence spectroscopy. Three-way data matrices were generated by acquisition of spectra as a function of the pH (between 2 and 11) and of different relative concentrations of the three components. The PARAFAC trilinear model, without restrictions and using one factor per metabolite, was used in the data analysis. A full decomposition of the data matrices into the spectra, concentration and pH profiles was obtained. This result shows that molecular fluorescence spectroscopy can be used for the development of robust analytical methods for the simultaneous determination of the three major metabolites of acetylsalicylic acid in complex background samples.     

Sustained blood concentration of salicylic acid following rectal administration of salicyluric acid in dogs

The blood concentrations of salicyluric acid and salicylic acid following rectal, intravenous and oral administrations of salicyluric acid (5, 10 and 60 mg/kg, respectively: salicylic acid equivalent) were determined in dogs. After rectal administration, a small amount of salicyluric acid was absorbed in intact form. The rest was hydrolyzed to salicylic acid, which was subsequently absorbed. The blood concentration of salicylic acid was maintained at 0.4-0.7 microgram/ml from 2 to 12 h. Following intravenous administration of salicyluric acid, salicyluric acid was detected in the blood but was rapidly eliminated. A trace amount of salicylic acid was detected, suggesting that systemic de-conjugation of glycine was involved. After oral administration of salicyluric acid, salicyluric acid was well absorbed. Salicylic acid was detected at low concentration for 12 h. Species difference in the metabolic fate of salicyluric acid in dogs, rabbits, rats and humans reported previously is discussed.     

Rapid and sensitive determination of acetylsalicylic acid and its metabolites using reversed-phase high-performance liquid chromatography

A rapid and sensitive high-performance liquid chromatographic technique was developed for the simultaneous determination of gentisic acid, salicyluric acid, acetylsalicylic acid and salicylic acid in plasma and serum. The method involved a single deproteinization step and separation using a reversed-phase column eluted with a buffered methanol (35%) mobile phase. Detection was achieved with a variable-wavelength ultraviolet detector set at 235 nm and a given chromatographic analysis could be completed in less than 10 min. The method was tested in both human and animal (rat) models given a single dose of acetylsalicylic acid.     

Determination of Aspirin,Salicylic Acid,Salicyluric Acid,and Gentisic Acid in Human Plasma and Urine by High Pressure Liquid Chromatography

Abstract

A method has been developed to simultaneously determine aspirin, salicylic acid, salicyluric acid, and gentisic acid concentrations in human plasma and urine. An extraction and dry-down step prepare the sample for resolution by reverse-phase high pressure liquid chromatography. The column effluent is monitored by both ultraviolet absorbance and fluorescence to optimize sensitivity and specificity for the compounds of interest.     

Amperometric biosensor for the quantification of gentisic acid using polyphenol oxidase modified carbon paste electrode

The affinity of mushroom polyphenol oxidase (PPO) towards gentisic acid (GA), a metabolite of acetyl salicylic acid (ASA), is demonstrated by spectrophotometry and by electrochemical techniques. The enzyme can selectively recognize GA even in the presence of large excess of ASA and its metabolic derivatives (salicylic acid (SA) and salicyluric acid (SUA)). At -0.150 V, the sensitivity is (6.1+/-0.1)x10(4) NAM(-1), the response is linear up to 2.0x10(-4) M and the detection limit is 5.0x10(-5) M. The kinetic parameters, obtained from Eadie-Hofstee plots, are I(max)=51.4 nA and K(m)(app)=6.7x10(-4) M.     

High Pressure Liquid Chromatographic Assay for Salicylic Acid and its Metabolites in Rat Urine

Abstract

An HPLC method for the determination of salicylic acid (SA), gentisic acid (GA), salicyluric acid (SU), and salicyl acyl glucuronide (SAG) in rat urine was developed. The method consisted of extracting SA, GA, and SU from acidified urine into 50:50 mixture of ethyl acetate and butyl chloride. Salicyl acyl glucuronide was extracted from neutral urine after conversion to salicyl hydroxamic acid with hydroxylamine. Salicyl phenolic glucuronide was estimated indirectly as the difference between total salicylate and sum of the four constituents mentioned above. Chromatographic separation was done on a C₁₈ column with U.V. detection at 310 nm using a mobile phase consisting of 5–10% acetonitrile in 3% glacial acetic acid. The extraction recovery of these compounds from spiked urine ranged from 90–108%. The detection limits were 10 μg/ml for GA, SU and SA, and 2.5 μg/ml for SHA. The method was applied to the study of salicylic acid metabolism in the rat.     

Simultaneous Determination of Salicylic Acid and Salicyluric Acid in Plasma and Urine by High Pressure Liquid Chromatography

Abstract

A sensitive, rapid, and specific high pressure liquid chromatographic (HPLC) assay was developed for the determination of salicylic (SA) and salicyluric (SU) acids in plasma and urine. The compounds are extracted into ethyl ether at acid pH, evaporated, and reconstituted prior to instrumental separation. Overall recovery of both compounds is 90 ± 5%, and the sensitivity limits are 150 ng of SU and 300 ng SA per ml of biological fluid. The assay was used for the determination of both compounds in plasma and urine of man following oral doses of 40 mg/kg of sodium salicylate.     

Determination of xylometazoline in plasma and urine by gas chromatography using a fused-silica capillary column and an electron-capture detector

A sensitive method is described for the determination of unchanged xylometazoline in plasma and urine at concentrations down to 35 nmol/l. After addition of naphazoline as an internal standard, both compounds are extracted with dichloromethane-diethyl ether (20:80) at pH 10, back-extracted with an acidic solution and re-extracted from a sodium hydroxide solution with dichloromethane-diethyl ether (20:80). The compounds are then derivatized with heptafluorobutyric anhydride in the presence of pyridine. The derivatives are determined by capillary gas chromatography using electron-capture detection.     

Chromatographic Studies of 34 Organic Acids on Papers Impregnated with Hydroxides of Aluminium and Cadmium

Abstract

Papers impregnated with aluminium hydroxide and cadmium hydroxide have been used for the chromatographic separation of organic acids exist in various biological materials, soil and water. The following important separations: cinnamic acid from hippuric acid; benzoic and m-nitrobenzoic acids from gallic, β-naphthalene acetic, β-naphthoxy acetic, phthalic, quinic and salicylic acids; and salicylic acid from citric, cis-aconitic, malic, quinic, tartaric and trans-aconitic acids can be achieved in common electrolytes (Cd(NO₃)₂, KI, NaCl, NH₄Cl) solution.

Hydroxides¹ show amphoteric behaviour i. e. they may exchange either cations or anions depending upon the pH of the solution, and t h i s may be shown by the following ionic equilibria.     

Simultaneous determination of active ingredients in ethnomedicine Gaultheria leucocarpa var. yunnanensis and its medicinal preparation by capillary electrophoresis with electrochemical detection

A simple and rapid capillary electrophoresis (CE) with electrcochemical detection (ED) method has been established for the simultaneous determination of seven active ingredients in the stems and roots of Gaultheria leucocarpa var. yunnanensis and its medicinal preparation, including (+)-catechin, rutin, gentisic acid, vallinic acid, salicylic acid, quercetin, and protocatechuic acid. The effects of working potential, pH, and concentration of running buffer, separation voltage, and injection time on CE-ED are systematically investigated. Under the optimum conditions, the seven analytes could be completely separated within 23 min in a borax running buffer (pH 8.7). A good linear relationship is obtained over three orders of magnitude with detection limits (signal-to-noise ratio=3) ranging from 5x10(-8) g/mL to 3x10(-7) g/mL for the analytes. The proposed method is successfully used in the analysis of real samples after a relatively simple extraction procedure, and the assay results are satisfactory.     

毛细管区带电泳法测定油田水中的脂肪酸

采用二硝基本甲酸一十六烷基三甲基溴化脓缓冲体系对油田水中短链脂肪酸进行了分析。应用间接紫外法,使脂肪酸在数分钟之内得以分离检测。研究表明,当缓冲溶液pH值为9.0、电解质浓度为5.0mmol／L、表面活性剂浓度为0.5mmol／L和甲醇含量为5％时可达到最佳的分高效果。     

Separation gallium-fer en presence d'edta

Macro- or microquantities of gallium can be separated from iron by precipitating the latter with sodium hydroxide in the presence of EDTA. Nearly all the gallium remains in solution. After the separation of iron, gallium is extracted with tributylphosphate from 3 N hydrochloric acid medium, and then re-extracted into water. Gallium is finally determined by precipitation with cupferron and ignition to the oxide, or for trace amounts of gallium, by colorimetric determination with rhodamine B. The method was checked with radioactive gallium and iron.     

硅钙合金中钙、铝的联合测定

硅钙合金用硝酸、氢氟酸溶解后，加入高氯酸并加热至冒烟以驱除氟，然后定容。移取两份样品溶液，一份中加入三乙醇胺溶液掩蔽铁、铝等干扰离子，再加入氢氧化钾溶液，使pH=12，用EDTA容量法测定钙。另一份中加入铁标准溶液、混合显色液（Zn-EDTA与络天青S的混合溶液）及六次甲基四胺缓冲溶液，用光度法测定铝。方法简便，结果准确、可靠。     

Solvent extraction of microgram amounts of magnesium with 8-quinolinol and tetrabutyl-ammonium iodide followed by spectrophotometry with chlorophosphonazo-III

A rapid and sensitive solvent-extraction procedure for the separation of magnesium is reported. Microgram (0.1–10) amounts of magnesium are extracted with a chloroform solution of 8-quinolinol and tetrabutylammonium iodide in the presence of tartrate and phosphate. Magnesium is then back-extracted into an aqueous buffer solution (pH 7.3; tetrabutylammonium hydroxide—boric acid) and determined spectrophotometrically using chlorophosphonazo-III. Up to 500 mg of sulphate, phosphate or cyanide, 200 mg of chloride, 20 mg of aluminum, barium or silicate, and 2 mg of calcium can be tolerated.