Determination of three anabolic compounds in calf urine by liquid chromatography with photodiode-array detection

A method for the determination of three anabolic hormones (diethylstilbestrol, dienestrol and trenbolone) in calf urine is described. After enzymatic hydrolysis, the samples were cleaned up by C18 solid-phase extraction. Drugs were extracted with hexane and analyzed by isocratic elution on a Discovery RP-Amide C16 5 microns column with photodiode-array detection at 240 and 347 nm. Both retention time and UV spectra were used for identification. Detection limits for the HPLC system were calculated to be 0.3 ng injected for all analytes in the standard mixture. However, for urine samples these limits increased because of the presence of unidentified matrix components. After extraction from urine, the limits of detection for the whole analytical procedure were 5 and 10 ng injected for trenbolone and stilbenes, respectively. The average recoveries of the hormones from spiked samples were in the range 53.1-56.7% with RSD between 11.3 and 14.5% for the whole procedure in the concentration range 25-2.5 ng ml-1.     

Determination of organolead compounds by liquid chromatography with on-line extraction and ultraviolet detection

Detection limits by ultraviolet detection in liquid chromatography (LC) for organolead species are improved by the use of a post-column, on-line, continuous liquid-liquid extraction system. Extraction of the organolead species is followed by membrane separation of the extracts from the aqueous mobile phase. Optimization of the merobrane used in the phase separator, ratios of aqueous-to-organic flow rates, extractor dimensions and shape, aqueous salt content, the detection wavelength, and other operational parameters are described. Improvements of detection limits over conventional LC methods with ultraviolet detection range from a factor of 2 for triethyllead chloride, up to a factor of over 10 for trimethyllead chloride. Calibration plots are linear over several orders of magnitude. Extraction efficiencies as a function of the organic extractant flow rate are discussed. The optimized approach is applied to spiked, distilled-water samples.     

Determination of capsaicinoids in peppers by microwave-assisted extraction-high-performance liquid chromatography with fluorescence detection

In this study, a simple method for the determination of free fatty acids, phytosterols, tocopherols, mono and diglycerides present in canola oil deodorizer distillate (DD) and soapstock samples was developed. Analytes were derivatized “in situ” using a mixture of hexamethyldisilazane (HMDS), pyridine and trifluoroacetic acid; separated by gas chromatography (GC) with mass spectrometry (MS) for final detection. Two drying procedures were evaluated for drying deodorizer distillate samples before derivatization: freeze drying and drying at 100 °C for 24 h. The use of high temperatures caused the degradation of tocopherols and phytosterols, while lyophilization did not affect the substances negatively. The chromatographic conditions used in this work allow for the separation and quantification of oleic, linoleic and linolenic acids, monoolein and monolinolein in both samples, and brassicasterol and α-tocopherol in deodorizer distillate samples. MS provided an accurate identification for the compounds which were at very low concentrations (>0.09%). Oleic acid was the most abundant compound in both samples. Deodorizer distillate was an important source of tocopherols which were not detected in the soapstock samples.     

Structure of hydroxycinnamic acid derivatives established by high-performance liquid chromatography with photodiode-array detection

Summary The present paper describes the development of a method for the differentiation of hydroxycinnamic acid derivatives by HPLC with photodiode-array detection. Furthermore spectral data of the compounds under investigation are given. Whereas p-coumaric acid derivatives are distinguishable from caffeic and ferulic acid derivatives by the positions of their spectrum maxima and their convexity interval value, it is not possible to distinguish between caffeic and ferulic acid derivatives because of overlapping spectrum maxima and convexity interval values.     

Structure of hydroxycinnamic acid derivatives established by high-perfomance liquid chromatography with photodiode-array detection

Summary The present paper describes the development of a method for the differentiation of hydroxycinnamic acid derivatives by HPLC with photodiode-array detection. Furthermore spectral data of the compounds under investigation are given. Whereas p-coumaric acid derivatives are distinguishable from caffeic and ferulic acid derivatives by the positions of their spectrum maxima and their convexity interval value, it is not possible to distinguish between caffeic and ferulic acid derivatives because of overlapping spectrum maxima and convexity interval values.     

Analysis of heparins by size-exclusion and reversed-phase high-performance liquid chromatography with photodiode-array detection

High-performance liquid chromatography (HPLC) of heparins was carried out with on-line photodiode-array detection. Average molecular weights and molecular weight distribution were calculated using computer data acquisition and handling; size-exclusion chromatography was performed using different selective microparticulate columns and narrow molecular weight distribution heparin standards for calibration; heparin peak purity was investigated using several methods for evaluation. Additional UV-absorbing compounds present in heparin preparations were characterized and quantitated by reversed-phase HPLC. These methods are useful for the analysis of the molecular weight distribution and peak purity of heparins and for the determination of additional drugs, additives or impurities.     

Analysis of cephalexin from canine skin biopsy by liquid chromatography with ultraviolet-visible photodiode-array detection

A sensitive and selective ion-paired liquid chromatographic method with UV-VIS photodiode-array detection was developed to measure cephalexin in skin biopsy samples. The method involved a sonication of minced canine skin with ethanol-acetonitrile-water (30:20:50, v/v/v) and ultrafiltration of received extract through 10,000 daltons. Separation of cephalexin from other components was by liquid chromatography using a reversed-phase column which was eluted with an ion-paired acetonitrile-water solution. Detection was achieved with a UV-VIS photodiode-array detector scanning from 230 to 320 nm. Cephalexin in the eluate was quantitated at its wavelength maximum of 260 nm. The evaluation of chromatographic peak homogeneity was performed by absorbance ratios, contour maps, first-derivative spectra and a three-dimensional spectrochromatogram. Additionally, the cephalexin peak identity was confirmed by liquid chromatography-mass spectrometry.     

Determination of valproic acid by high-performance liquid chromatography with photodiode-array and fluorescence detection.

The derivatization of valproic acid and undecylenic acid with 4-bromomethyl-7-methoxycoumarin is described. The derivatives were detected by photodiode-array and fluorescence detectors. The optimum monitoring conditions and the stability of the suspension solution and derivatives were investigated. A high-performance liquid chromatographic (HPLC) method with isocratic or gradient elution has been established for the analysis. This method has been used for the determination of total and free valproic acid in serum. There is a satisfactory correlation between the results obtained by this HPLC method and those measured by the enzyme immunoassay. Some other common anti-epileptic drugs did not interfere with the analysis. The method is simple and fast and has better sensitivity and linearity than enzyme immunoassay. It is suited for routine therapeutic drug monitoring.     

Determination of quinolones in animal tissues and eggs by high-performance liquid chromatography with photodiode-array detection

A rapid, specific reversed-phase HPLC method is described, with solid-phase extraction, for assaying five quinolones (ciprofloxacin, difloxacin, enrofloxacin, norfloxacin and marbofloxacin) with confirmative diode-array detection in samples of bovine kidney, muscle and eggs. The least efficient extraction was marbofloxacin from kidney tissue (64%). The lower detection limit for each quinolone was: enrofloxacin and ciprofloxacin, 1 ng; norfloxacin and difloxacin, 2 ng; marbofloxacin, 4 ng injected. The intra-day relative standard deviations were lower than 7.9% and lower than 8.6% for inter-day assays. These results indicate that the developed method had an acceptable precision.     

Comprehensive screening procedure for diuretics in urine by high-performance liquid chromatography

A rapid and reliable screening procedure using high-performance liquid chromatography for the detection of 23 diuretics (belonging to five different pharmacological groups) in urine has been developed. Two aliquots of 2-ml urine samples were extracted separately under acidic and basic conditions. The acidic and basic extracts were pooled, evaporated to dryness and reconstituted in methanol. The methanolic extract was injected onto a Hewlett-Packard Hypersil ODS C18 (5 microns) column (column I) and a Hewlett-Packard LiChrosorb RP-18 (5 microns) column (column II; an alternative column). The same gradient mobile phase was used for both columns. A diode array ultraviolet detector was set to monitor the signal to the integrator (Chem Station) at 230 and 275 nm. Recovery studies of the 23 diuretics were performed under acidic and basic conditions. The overall lower limits for detection on column I using both extraction procedures ranged from 0.5 to 1.5 micrograms/ml of urine (average 1.0 micrograms/ml). Amiloride, ethacrynic acid and probenecid could not be detected below 5 micrograms/ml of urine. No interference from the biological matrix was apparent. Amiloride could be detected in urine 4 h after oral administration of 15 mg of amiloride to a healthy volunteer, when the sample was extracted under alkaline conditions. The suitability of the screening method for the analysis of urine samples was tested by studying the variation with time of chlorthalidone, furosemide, probenecid, acetazolamide, quinethazone, spironolactone, bendroflumethiazide, bumetanide, triameterene and hydrochlorothiazide concentrations in the urine of normal human volunteers after minimum single or multiple (probenecid) doses.(ABSTRACT TRUNCATED AT 250 WORDS)     

Determination of psychotropic phenylalkylamine derivatives in biological matrices by high-performance liquid chromatography with photodiode-array detection.

Several procedures using high-performance liquid chromatography with photodiode-array detection have been developed to create phytochemical and toxicological profiles of phenylalkylamine derivatives in biological samples (e.g. plant materials and urine). Mescaline-containing cactus samples were extracted with basic methanol, using methoxamine as internal standard; the extraction and clean-up of urine samples were performed on cation-exchange solid-phase extraction columns. The extracts were separated on a 3-micron ODS column with acetonitrile-water-phosphoric acid-hexylamine as the mobile phase. Peak detection was performed at 198 or 205 nm; peak identity and homogeneity were ascertained by on-line scanning of the UV spectra from 190 to 300 nm. The detection limit of phenylalkylamine derivatives in urine and cactus material was 0.026-0.056 micrograms/ml and 0.04 micrograms/mg, respectively. Following a single oral dose of 1.7 mg/kg methylenedioxymethylamphetamine (MDMA) the concentrations found in urine ranged from 1.48 to 5.05 micrograms/ml MDMA and 0.07-0.90 micrograms/ml methylenedioxyamphetamine (a metabolite of MDMA). The mescaline content of the cactus Trichocereus pachanoi varied between 1.09 and 23.75 micrograms/mg.     

Stability-indicating hydrophilic interaction liquid chromatography method for highly polar and basic compounds

A hydrophilic interaction liquid chromatography (HILIC) method was developed for the analysis of very polar and basic 4-(aminomethyl)pyridine (4-AMP) and its related compounds. Separation parameters such as stationary phase, buffer pH, buffer ionic strength, organic modifier, and column temperature were evaluated. The retention mechanisms were explored through the evaluation of the common chromatographic parameters in the method development. The data indicated the existence of surface adsorption phenomena for 4-AMP and its positional isomers (2-AMP, 3-AMP). For two degradants, different retention mechanisms might be involved when compared to 4-AMP. The selectivity of two critical pairs 3-/4-AMP isomer and Degradant-1/-2 diastereomer changed through isoelution temperature with reversal of elution order. The validation results indicated that the HILIC method is a sensitive, reproducible, and robust method suitable for the analysis of 4-AMP and its related compounds.     

Algorithms for the assessment of peak purity in liquid chromatography with photodiode-array detection. Part II

Two modifications of the algorithm based on the Gram-Schmidt orthogonalization technique for the assessment of peak purity are presented. The performance of this approah is investigated for liquid chromatography with photodiode-array detection (LC-DAD) data, although its applicability is not restricted to this experimental model. This method is applied to simulated and experimental data where two compounds are eluting, but can be applied when more compounds are eluting. The results are compared with the ones obtained previously with the first version of this algorithm.     

The analysis of organic mercury compounds using liquid chromatography with on-line atomic fluorescence spectrometric detection

A new method for the analysis of organic mercury compounds is reported. The organomercurials are separated by high-performance liquid chromatography (HPLC). The compounds are converted to mercury(0) in a continuous-flow system by means of an oxidizing and a subsequent reducing solution. The elemental mercury generated is swept into the cell of an atomic fluorescence spectrometer (AFS) by a stream of argon. The compositions of the oxidizing solution, which contains peroxodisulphate and copper(II) in dilute sulphuric acid, and the reducing solution, which contains alkaline tin(II) chloride, were optimized, as were the gas–liquid separator (GLS), the condensing system and the geometry of the reaction coils. The method is applied to extracts of certified reference material (CRM) and to river sediments. High concentrations of methylmercury were found in the sediment samples. At one location, the presence of ethylmercury is derived from the sample chromatogram.     

Selenium speciation by high-performance liquid chromatography with on-line detection by atomic absorption spectrometry

Several approaches to the determination of selenomethionine, selenocystine, selenite and selenate by high-performance liquid chromatography with online detection by atomic absorption spectrometry are described. The N?2,4-dinitrophenyl derivatives of selenomethionine, selenoethionine, selenocystine and phenylmercury(II) cystineselenoate were recovered from aqueous solution, separated on a Nucleosil 5-NO₂ reversed-phase HPLC column with a methanolic mobile phase containing acetic acid and triethylamine, and detected with a quartz thermochemical hydride-generating interface–atomic absorption spectrometry (AA) system. The restriction of having to perform chromatography with an organic mobile phase (to support the combusion process) was overcome with a new interface design capable of operation with either organic or aqueous HPLC mobile phases. Using aqueous acetic acid (0.015% v/v) containing 0.1% (w/v) ammonium acetate delivered at 0.5cm³ min^?1, selenate, selenite, selenomethionine, selenocystine and selenoethionine were separated virtually to baseline on a cyanopropyl-bonded phase HPLC column. Other selenium compounds which were investigated included methane seleninic and methane selenonic acids as well as the crude oxidation product mixtures resulting from the treatment of selenomethionine and selenocystine with hydrogen peroxide. A procedure for extracting selenate, selenite, selenomethionine, selenocystine and selenoethionine from spiked water or ground feed supplement into liquefied phenol resulted in acceptable recoveries for the latter four analytes but was unacceptably low for selenate.     

Determination of cisplatin and related platinum complexes in plasma ultrafiltrate and urine by high-performance liquid chromatography with on-line radioactivity detection

A reversed-phase ion-pair chromatographic method with on-line radioactivity detection for the simultaneous determination of 195mPt-labelled cisplatin and related platinum complexes has been developed. With this system a good resolution of various radiolabelled platinum complexes can be achieved. The detection limit of the radioactivity detector is 10 ng of cisplatin (specific activity of 15 MBq/mg cisplatin) per millilitre of urine or plasma ultrafiltrate. The detector response is independent of both the chemical structure of the platinum complexes and the matrix composition of the samples. This method may serve as a reference system for other high-performance liquid chromatographic systems with less specific and sensitive detectors.     

Identification and determination of sulphamethazine and N4-acetylsulphamethazine in meat by high-performance liquid chromatography with photodiode-array detection

A simple and selective method for the determination of sulphamethazine (SMT) and its metabolite, N4-acetylsulphamethazine (N4-AcSMT), in meat by high-performance liquid chromatography (HPLC) with photodiode-array detection was developed. The drugs were extracted from meat with 0.2% metaphosphoric acid-methanol (6:4), followed by a Bond-Elut C18 clean-up procedure. The HPLC separation was carried out on a Supersphere RP-18e column (125 X 4.0 mm I.D.) using 0.05 M sodium dihydrogenphosphate (pH 4.5)-acetonitrile (8:2) as the mobile phase at a flow-rate of 0.5 ml/min, and monitored with a photodiode-array detector. The recoveries of SMT and N4-AcSMT from meat fortified at 0.5 micrograms/g were 90.1-93.3 and 93.0-94.4%, respectively, with coefficients of variation of 1.9-3.2 and 1.5-2.7%. The limits of detection were 0.02 micrograms/g for each drug. SMT was found in ten samples of imported meat (12.5%) at levels ranging from 0.05 to 1.05 micrograms/g.