Determination of Flecainide in Human Plasma by High Performance Liquid Chromatography with Fluorescence Detection

Abstract

A simple, rapid, selective, and sensitive high-performance liquid chromatographic (HPLC) method for the monitoring of plasma flecainide levels in a therapeutic or research environment is described. The drug is first separated from plasma by a single-step extraction with hexane and then quantitated by HPLC with fluorescence detection. Two linear ranges have been established; 100–2000 ng/ml for drug monitoring in clinical management of patients and 3–300 ng/ml for pharmacokinetic studies. The intra-day variation is less than 6%.     

Fluorometric Determination of Iron(Iii) with O-Hydroxyhydroquinonephthalein in the Presence of Brij 58

Abstract

A highly sensitive fluorescence reaction of iron(III) with o-hydroxyhydroquinonephthalein (Qnph) in the presence of various surfactants, and its application to the fluorophotometry of trace amounts of iron(III) is described. the method is based on the fluorescence quenching reaction between Qnph and iron(III) in the presence of Brij 58 at pH 3–4. the quenching calibration graph was linear over the range 0 – 300 ng per ml iron(III) by using fluorescence reaction at Em 525 nm with Ex 470 nm, and the iron(III) detection limit was 5 ng/ml. the proposed method is simple, rapid and does not involve heating or solvent extraction.     

High Performance Liquid Chromatographic Assay of Methoclopramide in Plasma Using a Silica Gel Column and An Aqueous Meobile Phase

Abstract

A high performance liquid chromatographic method for quantitating matoclopramide in plasma is presented. Proteins ara precipitated from the plasma sample with acetonitri la containing the internal standard, procainamida. The treated samples ara than analyzad using an Ultrasphere Si column, an aqueous solution at pH 7 of 65% CH³CN and 5.0 mM (NH₄)₂HPO₄ as a mobile phase, and a fluorescence detector. The retention times for drug and intarna1 standard ara 11.2 and 13.2 min, respectively. The caibration curve is Linear from 0.89 to 44.5 ng/ml. The detection limit is 0.89 ng/ml [signaL/hoisa = 31] for 0.2 ml plasma samples Pracision is measured by intraday and intarday coefficients o f variation, which are less than 10%. This method is currently being used for pharmacokinetic studies of methoclopramide.     

The Determination of a New Trifluorinated Quinolone,Fleroxacin, Its N-Demethyl,and N-Oxide Metabolites in Plasma and Urine by High Performance Liquid Chromatography with Fluorescence Detection

Abstract

A liquid chromatographic method is described for the determination of the new fluoroquinolone Ro 23–6240 and its N-demethyl and N-oxide metabolites in plasma and urine. The three substances were extracted from aqueous solution with dichloromethane/isopropanol containing sodium dodecyl sulphate. After evaporation and reconstitution, samples were analysed on a reversed-phase column using ion pair chromatography and fluorescence detection. The limit of quantification was 10–20 ng/ml (RSD 4%) using a 0.5 ml plasma sample, and the inter assay precision was 3–10% over the concentration range 50 ng/ml to 20 μg/ml. Recovery from plasma was 81% (RSD 10%) over the range 10 ng/ml to 5 μg/ml. The method has been applied successfully to the analysis of several thousand samples from human pharmacokinetic studies. Care has to be taken to avoid exposure of samples to direct sunlight, and the use of opaque vessels for sample storage and handling is recommended.     

A New Fluorimetric Method for the Determination of Ascorbic Acid

Abstract

The fluorescent reaction between ascorbic acid(AA) and 2-cyanoacetamide was studied. The experimental results showed that AA can react with 2-cyanoacetamide at pH 12.9–13.3, and form a fluorescent product, which emitted strong fluorescence. The fluorescence intensity was measured at excitation and emission wavelengths of 329 and 380nm, respectively. A linear relationship was obtained between the fluorescence intensity and AA concentration in the range of 0.1–50μg/ml, the regression coefficient is 0.9994, and the detection limit of AA is 0.03μg/ml. (signal-to-noise=3).     

Determination of Nucleic Acids Using Rivanol as the Fluorescent Probe in the Presence of SDS

ABSTRACT

The quantitative method for nucleic acids using rivanol as the fluorescent probe in the presence of SDS was proposed. Under proper conditions, addition of nucleic acids to a mixture of rivanol and SDS resulted in enhanced fluorescence and spectral shifts of rivanol-SDS system. The calibration graph was linear in the range of 0–10.0 μg/ml for CT DNA and 0–9.0 μg/ml for yeast RNA, the limit of detection was 62 ng/ml for CT DNA and 156 ng/ml for yeast RNA. CT DNA could be determined in the presence of 20%(w/w) yeast RNA.     

Sodium Coumarin 6-Sulfonate,A Fluorometric Ion-Pairing Reagent for Tertiary Amines. Application to the Determination of Chlorpheniramine Maleate

Abstract

A study of sodium coumarin 6-sulfonate as a fluorescent ionpair reagent indicated that it could be useful in the analysis of tertiary amines such as chlorpheniramine maleate. The physical properties of the coumarin sulfonate that make it suitable as a fluorescent ion-pair reagent for basic drugs are its high relative quantum yield (0.76) and its acidity (pKa of ?7.66). Methylene chloride containing 5% n?pentanol was used to extract the coumarinchlorpheniramine ion-pair from aqueous solution. It was found that a 10^?2 M coumarin concentration yielded a 92% recovery of chlorpheniramine at pH 5. Following phase separation, the coumarin species was completely ionized by the addition of tetrabuty1 ammonium hydroxide to the organic phase. After irradiation for 30 min using long wavelength ultraviolet light (365 nm), the fluorescence intensity of the sample was measured using excitation and emission wavelengths of 400 and 540 nm, respectively. Comparison of fluorescence data of spiked aqueous samples to that of a chlorpheniramine maleate standard curve performed concurrently gave drug concentration in the samples. The calibration curve was linear in the 50–1000 ng/ml range (0.13 ? 2.6 × 10 ^?6 M). The procedure allowed the determination of chlorpheniramine maleate with an accuracy of 4–6% and a precision of 2–6% RSD (relative standard deviation). The minimum detectable concentration of drug (S/N = 2) that can be assayed by this method is 50 ng/ml of the maleate salt (35.3 ng/ml of chlorpheniramine free base).     

Routine Determination of a New 1–4 Dihydropyridine,Oxodipine, in Human Plasma by High Performance Liquid Chromatography with Electrochemical Detection

Abstract

A rapid, specific and reproducible high-performance liquid chromatographic routine assay with electrochemical detection was developed for the determination of Oxodipine in human plasma.

After extraction at alkaline pH by cyclohexane, Oxodipine and its internal standard were chromatographied on a reversed-phase column.

Calibration curves were linear over a concentration range of 1–50 ng/ml with relative errors within-day or between-day not exceeding 8% at any level.

The limit of detection was 30 pg injected based on a signal-to- noise ratio of 7. However, the reliable limit of quantification was 1 ng/ml using 1 ml of human plasma.

A dual-electrode coulometric detector was operated in a screening mode of oxidation, providing a greater specificity and reducing background noise.

This method allowed the complete follow-up of clinical pharmacokinetic studies and drug monitoring in patients.     

Voltammetric Determination of Aluminium in Haemodialysis Concentrates Using the Adsorption of the Al(III)-1,2-Dihydroxyantraquinone-3-sulphonic Acid Complex in Presence of Calcium

Abstract

This paper describes a method for the quantitative determination of aluminium in haemodialysis concentrates, based on the adsorption on a static mercury drop electrode of the Al-1,2 dihydroxyantraquinone-3-sulphonic acid complex. The signal was notably increased in presence of calcium. The electrolysis was carried out at -0.900 V. After 60 sec the aluminium contents were measured by differential pulse voltammetry. In these conditions aluminium can be determined in the range 0.65–38 ng/ml with a detection limit (3[sgrave]) of 0.20 ng/ml. The relative standard deviation was in all instances less than 2.1%.     

Analysis of Indenolol In Biological Fluids By High Performance Liquid Chromatography

Abstract

The analysis of indenolol in plasma and urine is described. The method involves extraction of the drug from plasma or urine using chloroform at basic pH. The separation was performed on CN column using methanol and 0.01M potassium dihydrogen phosphate solution 50:50. The efficiency of extraction was 97%. Minimum detectable amount by fluorescence was 20 ng/ml.     

High Performance Liquid Chromatographic Determination of Amiodarone in Plasma and Tissues

Abstract

A simple and rapid high-performance liquid chromatographic (HPLC) method for the determination of amiodarone (AD) in plasma and tissues was developed. The method involved deproteinization of plasma or homogenized tissue with acetonitrile containing an internal standard (N-Cetylpyridinium chloride) followed by reversed phase chromatography using μ bondapack C₁₈ column (10μm) with a mobile phase consisting of acetonitrile - methanol - sodium dihydrogen phosphate buffer (70:10:20%, v/v), the pH adjusted to 4.0 and pumped at flow rate of 1.0 ml/min. The column effluent was monitored at 242 nm. A linear relationship was obtained between peak height ratios (drug to internal standard) versus drug levels over the concentration range of 50–750 ng/ml. The detection limit of AD in plasma and tissues by this method was 20 ng/ml.     

Multiresidue Analysis of Pesticides in Water from Rice Cultures by On-line Solid Phase Extraction Followed by LC-DAD

Abstract

An automated on-line solid phase extraction procedure followed by liquid chromatography with diode array detection was investigated for the determination of different classes of pesticides in water samples containing varied amount of humic substances. The different pesticides used were: carbendazin, carbofuran, atrazine, diuron, propanil, molinate, alachlor, parathion-ethyl, diazinon, trifluralin and the degradation products deisopropylatrazine and deethylatrazine. Humic substances extracted from a Brazilian sediment were used from 5 to 80 mg/l and their influence on recoveries was evaluated in neutral and acidic media. Recoveries higher than 70% were obtained for all the pesticides, from the preconcentration of 75 ml of aqueous sample fortified at 2 ng/ml using precolumns packed with PLRP-S. Good recoveries were obtained at neutral pH for most of the analytes up to 40 mg/l of humic acid. Only at 80 mg/l the recoveries were significantly affected, both at acidic and neutral pH. The method was applied to the determination of pesticides in river water spiked at 0.1 to 1 ng/ml. Detection limits obtained for water containing 10 mg/l of humic acid were between 0.05 and 0.3 ng/ml.     

An Improved Method for the Determination of Reserpine in Plasma Using Liquid Chromatography with Fluorescence Detection

Abstract

A liquid chromatographic method coupled with fluorescence detection was developed to measure plasma reserpine concentrations. After extraction from 3 ml of plasma, the reserpine and internal standard (methyl-18-triethoxy benzoyl reserpate) residues were oxidized to their respective fluorophors by vanadium pentoxide and chromatographed on a reversed phase trimethylsilyl column. These compounds were detected at excitation wave length 460 nm and analyzed at 570 nm. The minimum quantifiable level was ca 0.3 ng/ml and the absolute recovery was determined to be between 78–83%. The coefficient of variation was less than 9% for day-to-day and within run analyses. This method is suitable for pharmacokinetic studies of reserpine in man.     

Separation and Removal of Mercury(II) from Water Samples Using (Acetylacetone)‐2‐Thiol‐Phenyleneimine Immobilized on Anion‐Exchange Resin Prior to Determination by Cold Vapor Inductively Coupled Plasma Atomic Emission Spectroscopy

Abstract

(Acetylacetone)‐2‐thiol‐phenyleneimine (H₂L) immobilized on an anion‐exchange resin (Dowex) was used for separation and removal of mercury from natural water samples and for preconcentration prior to its determination by cold vapor inductively coupled plasma atomic emission spectroscopy. The metal was eluted from the column using a solution of 10% thiourea in 0.1 M HCl. The modified resin is higly selective with an exchange capacity of 1.60 mmol g^?1. Various parameters like pH, column flow rate, and desorbing agents are optimized. The proposed method has a linear calibration range of 15–1000 ng/ml Hg(II), with a relative standard deviation at the 15 ng/ml level of 3.5%. The precision of the method (evaluated as the relative standard deviation obtained after analyzing six series of five replicates) was ±4.2% at the 50 ng/ml level of Hg(II). The method has been used for routine determination of trace levels of mercury species in natural waters. The potential application of modified resin for the removal of mercury(II) from two natural water samples (top water and lake water) spiked with 50 ng/ml of mercury (II) was studied by ICP‐AES, and the results proved that excellent percent extraction of mercury(II) from both natural water samples was obtained by column method using modified resin.     

Determination of Saccharin in Plasma and Urine by High Performance Liquid Chromatography

Abstract

A sensitive and specific high performance liquid chromatographic (HPLC) assay for the determination of saccharin in plasma and urine was developed. Saccharin is extracted into diethyl ether at acid pH, evaporated, and reconstituted prior to instrumental analysis. Overall recovery of saccharin is 86.9 + 8.6% and the sensitivity limits of detection is 0.15 μg per ml of plasma or urine using a fluorescence detector. The sensitivity limit in plasma can be extended to 20 ng per ml by use of a 2 ml assay volume and detector attenuation. The assay was used for the determination of saccharin in plasma and urine of rats following oral doses of 5 mg/kg.     

Flow Injection Analysis of Carboxylic Acid Drugs Using Cationic Dyes and On-Line Ion-Pair Extraction

Abstract

A flow injection system containing an on-line ion-pair extractor has been designed for the analysis of carboxylic acid drugs using either spectrophotometric detection with gentian violet as counterion or fluorescence detection with acridine orange. Salicylic acid, valproic acid, and ibuprofen were selected as model drugs. A mobile phase of 90:10 aqueous pH 7 phosphate buffer-absolute methanol was pumped through the system at 1 ml/min. A chloroform solution of the cationic dye was pumped into the mobile phase at 1.25 ml/min and the chloroform layer containing the dye-drug ion-pair separated prior to detection. Peak height and absorbance were linear for salicylic acid, valproic acid, and ibuprofen in the 0.5–10, 5–50, and 1–10 μg/ml ranges, respectively. Peak height and fluorescence were linear for salicylic acid, valproic acid, and ibuprofen in the 0.13–5, 2.5–50, and 0.5–20 μg/ml ranges, respectively. Accuracy and precision for the spectrophotometric assays were in the 2–6% and 3.3–6.6% ranges, respectively, and in the 0.3–4% and 1.3–5.4% ranges, respectively, for the fluorescence assays. Peak height and absorbance were also shown to be linear in the 16–500 μg/ml range for prostaglandin PGF_2α with accuracy and precision of 1–3% and 5–6%, respectively, for spiked samples. Commercial dosage forms containing valproic acid and ibuprofen were assayed by the spectrophotometric assay and found to be within acceptable USP limits. Spiked ibuprofen samples at the 5 and 10 μg/ml level were assayed using an octadecylsilane column inserted into the flow injection system. One to two percent accuracy and 2.5–5% precision were obtained for the drug using the FIA-column system.     

Rapid Determination of Bupropion in Human Plasma by High Performance Liquid Chromatography

Abstract

A high performance liquid chromatographic (HPLC) technique has been developed for the determination of bupropion hydrocloride (Bup) in human plasma, using a reversed-phase method, with UV detection at 250 nm.

The internal standard 5-(P-methylphenyl)-5-phenylhydantoin (MPPH), was used as an aid to quantitation. The plasma was deprotemized with acetonitrile and the clear supernatant was directly injected in the chromatographic system. The lower limit of quantitation was 5.0 ng/ml using only 100 μl of plasma sample.

Linear regression analysis for the calibration plots obtained on five different days over a two-week period for the the two ranges used (10–250 ng/ml and 250–2000 ng/ml) in plasma indicated excellent linearity and reproducibility. The mean recovery of spiked Bup in plasma samples over the concentrations studied was found 96.5 ± 3.14%.

The method revealed that more than 30% of Bup was lost when the supernatant was stored at room temperature for 24 hrs.     

Selective Determination of Cytosine Based on Its Fluorogenic Reaction with Triethylamine/Chloroacetonitrile

Abstract

A sensitive fluorometric method is described For selective determination of cytosine in nucleobases. The method is based on chemical derivatization of cytosine by triethylamine/chloroacetonitrile. The effects of solvent, reaction temperature, reaction time and concentration of reagents on the efficiency of the reaction were studied. A good linear relationship between fluorescence intensities and cytosine concentrations in the range of 2.0–800 ng/mt was observed. The detection limit for cytosine is 0.6 ng/ml (S/N=3). The relative standard deviations (7 replicates) for measurements of 50 and 500 ng/ml cytosine were 2.1 and 2.5%, respectively.     

Spectrofluorimetric Determination of Chlorpromazine Hydrochloride and Thioridazine Hydrochloride

Abstract

Fluorescence spectroscopy was applied to the development of a sensitive and simple method for the determination of chlorpromazine HCl and thioridazine-HCl. The method is based upon development of an intense fluorescence using N-bromosuccinimide as the fluorogenic reagent. The produced fluorescence has very characteristic excitation and emission spectra and was stable for at least one hour. The results were reproducible and as little as 5 ng/ml chloropromazine HCl and 1 ng/ml thioridazine-HCl could be determined. The method was applied successfully to the analysis of various commercially available dosage forms. The obtained results were in good agreement with those of the official BP 93 procedures.     

A Direct and Sensitive Method for the Determination of Salicylamide in Microplasma Samples by High-Performance Liquid Chromatography Using Fluorescence Detection

Abstract

A quantitative analysis of salicylamide in microplasma volumes by high-performance 1iquid chromatography using fluorescence detection is reported. The procedure is extremely simple and very rapid, involving the direct introduction of the plasma sample on the HPLC column. The assay procedure is linear over the concentration range studied, 0–100 ng/ml with correlation coefficient for the linear regression, r = 0.998. This assay procedure enables the detection of salicylamide as low as 5.0 ng/ml in plasma, using sample volume of 100 μl.