Determination of glyoxal and methylglyoxal in the serum of diabetic patients by MEKC using stilbenediamine as derivatizing reagent

An analytical method has been developed for the separation of glyoxal (Go), methylglyoxal (MGo), and dimethylglyoxal (DMGo) by MEKC using stilbenediamine (SD) as derivatizing reagent, separation time 6.5 min, SDS as micellar medium at pH 8, and sodium tetraborate (0.1 M) as buffer. Uncoated fused-silica capillary, effective length 50 cm x 75 microm id; applied voltage 20 kV and photodiode array detection, were used. Calibration was linear within 0.02-150 microg/mL with detection limits 3.5-5.8 ng/mL. Go and MGo, observed for diabetic and healthy volunteers, were within 0.098-0.193 microg/mL Go and 0.106-0.245 microg/mL MGo with RSD 1.6-3.5 and 1.7-3.4%, respectively, in diabetics against 0.016-0.046 microg/mL Go and 0.021-0.066 microg/mL MGo with RSDs 1.5-3.5 and 1.4-3.6%, respectively, in healthy volunteers. Go and MGo in diabetics were also measured by standard addition and DMGo as an internal standard. Additives do not contribute significantly to Go and MGo matrix.     

Capillary gas chromatographic determination of methylglyoxal from serum of diabetic patients by precolumn derivatization using meso-stilbenediamine as derivatizing reagent

Stilbenediamine is used as derivatizing reagent for methylglyoxal (MGo) and dimethylglyoxal for the gas chromatographic (GC) determination of MGo from the serum of diabetic patients and healthy volunteers. The derivatization is obtained at pH 3. GC elution and separation are carried out on an HP5 column (30 m x 0.32 mm i.d.) at column temperature 150 degrees C with a programmed heating rate of 50 degrees C/min up to 250 degrees C, and a total run time of 7 min. The nitrogen flow rate is 5 mL/min and detection is carried out by flame ionization detection. The linear calibration curves are obtained with a range of 0.076-0.760 microg/mL and the detection limit is 25 ng/mL MGo. The amounts of MGo found in the serum of healthy volunteers and diabetic patients are 0.025-0.065 microg/mL and 0.115-0.228 microg/mL, with coefficient of variation 1.3-3.1% and 1.4-3.3%.     

High-performance liquid chromatographic analysis of guanidino compounds using ninhydrin reagent. II. Guanidino compounds in blood of patients on haemodialysis therapy

An automated high-performance liquid chromatographic method using alkali-ninhydrin reagent for the post-column derivatization of guanidines has been developed. This procedure was applied to measurements made before and after haemodialysis. Among the guanidino compounds found in human blood, methylguanidine showed the lowest removal rate. The removal rate of guanidinosuccinic acid correlated with the plasma alpha 1-globulin fraction. The removal rate of each guanidino compound decreased with the period of dialysis.     

Activated carbamate reagent as chiral derivatizing agent for liquid chromatographic optical resolution of enantiomeric amino compounds

Summary A chiral derivatization reagent having activated succinimido carbamate moieties were developed for the optical resolution of enantiomeric amines by high-performance liquid chromatography. Succinimido R-(+)- or S-(–)-1-phenylethyl and R-(+)- or S-(–)-1-(-naphthyl)-ethyl carbamates were synthesized by the reaction of optically active phenylethyl and naphthylethyl amines with discuccinimido carbonate (DSC). These reagents reacted with both primary and secondary amine enantiomers such as amino acids and -amino alcohols to give the corresponding diastereomeric urea derivatives. These diastereomers were efficiently separated by reversed-phase liquid chromatography and detected by their absorption or the fluorescence of the chromophores. The chiral derivatization procedure was applied to the separation and determination of enantiomeric propranolol in serum.     

Fluorimetric determination of monosubstituted guanidino compounds with benzoin—dimethylformamide reagent

A sensitive fluorimetric method for the determination of monosubstituted guanidino compounds is based on their reaction in potassium hydroxide solution with benzoin in the presence of dimethylformamide. The fluorescence produced is stabilized by β-mercaptoethanol and shows excitation and emission maxima around 325 and 435 nm, respectively. The method is simple, selective for monosubstituted guanidino compounds, including polypeptides with one or two arginyl residues, and sensitive; compounds can be determined at concentrations as low as 0.08—0.22 nmol ml^-1.     

Gas chromatographic separation of optically active anti-inflammatory 2-arylpropionic acids using (+)- or (-)-amphetamine as derivatizing reagent

A method is described for the derivatization of several non-steroidal anti-inflammatory arylalkanoic acids (ibuprofen, ketoprofen, naproxen, fenoprofen, flurbiprofen, pirprofen, cicloprofen, tiaprofenic acid, etodolic acid) with optically active amphetamine. The usefulness of this reagent compared to alpha-methylbenzylamine is described. The enantiomers are separated as diastereoisomers using capillary gas chromatography with nitrogen-phosphorus detection. The procedure is readily applied to the quantification of the enantiomers in urine and plasma samples.     

Liquid chromatographic determination of vanadium in petroleum oils and mineral ore samples using 2-acetylpyridne-4-phenyl-3-thiosemicarbazone as derivatizing reagent

Liquid chromatographic method has been developed, based on precolumn derivatization of vanadium(V) with 2-acetylpyridine-4-phenyl-3-thiosemicarbazone (APPT). The complex is extracted in chloroform together with palladium(II), tin(II) and iron(III) and eluted and separated completely from Kromasil 100 C-18, 10 μm (25 cm × 4.6 mm i.d.) column with methanol:water:acetonitrile (60:30:10, v/v/v) with a flow rate of 1 ml/min. UV detection was at 260 nm. Linear calibration curve was obtained with 1-12.5 μg/ml vanadium(V) with detection limit of 8 ng/injection (20 μl). A number of metal ions tested did not affect the determination of vanadium. The test mixtures were analyzed for vanadium(IV) and vanadium(V) contents and relative% error was obtained ±1-8%. The method was applied for the determination of vanadium in petroleum oils and mineral ore samples with vanadium contents of 0.32-2.3 and 121.7-717.3 μg/g with R.S.D. of 1.5-4.5 and 0.38-4.7%, respectively. The results correlated with reported values and by atomic absorption spectrophotometry.     

Improved high-performance liquid chromatographic determination of guanidino compounds by precolumn dervatization with ninhydrin and fluorescence detection

Ninhydrin has been investigated as a pre-column derivatization reagent for guanidino compounds. The reaction takes place under strongly alkaline conditions, followed by a second step at low pH and elevated temperature. This procedure yields derivatives with favourable fluorescence properties (excitation at 390 nm, emission at 470 nm). Amino acids do not react with ninhydrin under these conditions so that the method can easily be used for biological samples. Reversed-phase HPLC separations of the derivatives of several representative guanidino compounds in human blood have been achieved with gradients consisting of aqueous formic acid and methanol. Fluorescence detection yields quantification limits of about 20 microg L(-1). Hyphenation with electrospray mass spectrometry has been used to confirm the identity of the derivatives.     

Liquid chromatographic determination of cobalt(II), copper(II) and iron(II) using 2-thiophenaldehyde-4-phenyl-3-thiosemicarbazone as derivatizing reagent

The complexing reagent 2-thiophenaldehyde-4-phenyl-3-thiosemicarbazone (TAPT) was examined for high performance liquid chromatographic (HPLC) separations of cobalt(II), copper(II) and iron(II) or cobalt(II), nickel(II), iron(II), copper(II) and mercury(II) as metal chelates on a Microsorb C-18, 5-mum column (150x4.6 mm i.d.) (Rainin Instruments Woburn, MA, USA). The complexes were eluted isocratically with methanol:acetonitrile:water containing sodium acetate and tetrabutyl ammonium bromide (TBA). UV detection was at 254 nm. The solvent extraction procedure was developed for simultaneous determination of the metals, with detection limits within 0.5-2.5 mug ml(-1) in the final solution. The method was applied for the determination of copper, cobalt and iron in pharmaceutical preparation.     

Electrode mechanism and voltammetric determination of selected guanidino compounds

The present review describes the recent results on the electrochemical activity of bio-guanidino compounds, such as famotidine, metformin, acyclovir, ganciclovir, zanamivir, moroxydine as well as guanidino compounds, such as S-[(2-guanidino-thiazol-4-yl)methyl]isothiourea hydrochloride, 2-guanidino-1,3-thiazole, 2-guanidinobenzimidazole. The focus is on analyzing the electrode mechanism of the guanidino compounds at the hanging mercury drop electrode and at the silver amalgam film electrode, as well as on the character of the square wave (SW) voltammetric signals. It has been stated, that the compounds can act as electrocatalysts — they are protonated and adsorbed at the surface of the electrode, after which the protonated forms of the compounds are irreversibly reduced, yielding their initial form and hydrogen. The experimental adsorption data obtained by measuring the differential capacity of the double layer, the zero charge potential, and the surface tension at the zero charge potential have established the adsorption processes underlying their electrochemical activity. The analytical application of the obtained voltammetric signals in the determination of these compounds in biological samples is also presented. This review concentrates on our own results in the context of general developments in the field.      

Gas chromatographic approach for the determination of carbonyl compounds in ambient air

In this study, an effort was made to apply gas chromatography (GC) with a flame ionization detector (FID) to the determination of gaseous carbonyls (without derivatization) at sub ppb level. A GC system interfaced with a multi-function thermal desorber system (TD) was hence tested for the collection and analysis of gaseous carbonyls. During this study, the calibration properties of five carbonyl compounds - acetaldehyde, propionaldehyde, butyraldehyde, isovaleraldehyde, and valeraldehyde - were evaluated by varying the operation conditions of the TD system (i.e., sample transfer approaches and sorbent types of cold trap). The results were generally discernible between compounds (light and heavy carbonyls) and/or between selected concentration levels. Most interestingly, the GC detection properties of the lighter aldehydes (acetaldehyde and propionaldehyde) varied significantly, as they were sensitively affected by the types of cold trap combination. However, the heavier aldehydes - butyraldehyde, isovaleraldehyde, and valeraldehyde - maintained highly constant trends for GC calibration. According to this study, a GC-based quantification of aldehydes can be completed by an optimized setup of TD system.     

Gas chromatographic determination of phenol compounds with automatic extraction and derivatization

Two gas chromatographic procedures for the determination of a variety of substituted phenols in water samples are described. The phenols were extracted or extracted-derivatized by using a continuous liquid-liquid extraction-derivatization system and quantified with flame ionization detection. Ethyl acetate was found to be the most efficient solvent for phenols whereas n-hexane yielded essentially the same recoveries for derivatized phenols. Between 0.1 and 300 mg/l of the different phenols can be detected with a relative standard deviation 1.1 and 3.7%. The acetate esters of six phenols were formed by the direct addition of acetic anhydride to the organic extractant. The stable acetate esters thus formed were isolated by using a standard dimethyl polysiloxane gas chromatographic column.     

Ion-exchange chromatographic separation and fluorometric detection of guanidino compounds in physiologic fluids.

A high-performance liquid chromatographic procedure has been developed for the separation and fluorometric detection of guanidino compounds in physiologic fluids. All guanidino compounds were separated on a 17 X 0.46 cm cation-exchange column using a stepwise pH gradient. The chromatographic system was designed to enable the use of the specific reagent 9,10-phenanthrenequinone as a means of monitoring the guanidino compounds of physiologic fluids. This new analytical method is so sensitive that it enables the analysis at the picomole level. Our automatic guanidino-compound analyzer was successfully applied to the quantitative determination of all guanidino compounds in physiologic fluids from normal controls and uremic patients.     

Reversed-phase liquid chromatographic separation of phenolic compounds with a new derivatizing reaction

Summary A reversed-phase HPLC method for resolution of phenoic compounds is presented. A new derivatization reaction has been developed employing diazotized 4-amino-benzonitrile, which reacts also with parasubstituted phenols. The products of the reaction can be extracted in n-butanol, allowing preconcentration and clean-up steps; the extracts are very stable and show strong absorption in the visible, where many interferences are avoided. The possibility of resolution of complex mixtures is discussed with reference to the use of reversed-phase columns using octadecyl- and phenyl bonded silica.     

Gas chromatographic determination of organolead compounds with an alternating current plasma detector

The performance of the gas chromatography/alternating current plasma detector as a selective detector for organolead compounds is investigated. The helium make-up flow rate and the spatial position from which the lead emission is viewed, have an effect on the detector response. The detection limit for tetrabutyl lead was established as 130 pg/s and the lead selectivity ratio was found to exceed 13,800. Some applications of organolead determination in complex matrices were also studied in order to demonstrate the selectivity and sensitivity of the alternating current plasma detector.     

Gas chromatographic determination of formaldehyde in air using solid-phase microextraction sampling

Summary The optimization of in situ derivatization and preconcentration of formaldehyde in air using solid phase microextraction with gas chromatographic determination was investigated. A dimethylpolysiloxane coating (7 μm) solid-phase microextraction needle was used in the final procedure as a support for derivatizing reagents such as 2,4-dinitrophenylhydrazine and acetylacetone. Standard concentrations of formaldehyde in air were obtained using a headspace technique and equilibrium concentrations of formaldehyde in air were calculated using Henry's law. After derivatization on the fiber, the derivative was thermally desorbed in the injector of a gas chromatograph and analyzed using an electron capture detector. A detection limit of 0.17 mg m⁻³ was obtained. Calibration was done at 296 K. Reproducibility of the method was 9.6%. Some real air samples were also analyzed. The method is very convenient and ideal for the rapid determination of formaldehyde in air. Presented at: Balaton Symposium on High-Performance Separation Methods, Siófok, Hungary, September 3–5, 1997     

High-performance liquid chromatographic determination of uranium using solvent extraction and bis(salicylaldehyde) tetramethylethylenediimine as complexing reagent

The reagent bis(salicylaldehyde)tetramethylethylenediimine has been used for the determination of dioxouranium(VI), based on complexation in aqueous solution at pH 6, followed by extraction in chloroform and HPLC determination on a Hypersil ODS (3 μm) column. The complex was eluted with the ternary mixture methanol-acetonitrile-water (40:30:30, v/v/v), with UV detection at 260 nm. Oxovanadium(IV), iron(III), copper(II), cobalt(II), nickel(II) and palladium(II) were completely separated and did not interfere in the determination of uranium. The linear calibration range and detection limits have been obtained. The method has been applied to the determination of uranium together with copper, iron and nickel in mineral ore samples.