Simultaneous High-Performance Liquid Chromatographic Assay of Acetaminophen,Acetylsalicylic Acid,Caffeine, and D-Propoxyphene Hydrochloride

Abstract

A reversed phase high-performance liquid chromatography (HPLC) method for simultaneous measurement of acetaminophen (I), acetylsalicylic acid (II), caffeine (III) and d-propoxyphene (IV), using phenacetin (V) as an internal standard was developed. Using a 6.5 μ C-8 reversed phase column (RPP) with a mobile phase consisting of 0.01M sodium acetate solution: methanol (85:15%) at pH 4.1 enabled the Chromatographic separation of the four components in about 12 min. Quantitation was achieved by measuring the peak height ratio of each component relative to the internal standard. the validity of the developed method was tested by analyzing laboratory-prepared mixtures containing the four components in various proportions. Assay precision and sensitivity have been established for each component. the developed method proved to be stability-indicating as it can be applied to monitor salicylic acid as a degradation product in acetylsalicylic acid samples.     

GLC and HPLC Determination of Diazepam and its Degradation Products in Pharmaceutical formulations

Abstract

Stability-indicating high performance liquid chromatographic (HPLC) and gas-liquid chromatographic (GLC) assays for diazepam in pharmaceutical formulations are described. In HPLC method, the material is extracted with 5 % aqueous methanol and chromatographed on a dimethyloctyl stationary phase using methanol-water-acetic acid (80: 20: 1) and propyl paraben internal standard. The system separated diazepam from the main degradation products, desmethyl diazepam (a synthetic precursor of diazepam) and the excipients present in ampoules and syrups. The GLC method included the extraction of diazepam and 2-methylamino-5-chiorobenzo-phenone (MACB) from aqueous acidic solution into chloro form leaving the other degradation products in the aqueous phase. The chloroform extract is evaporated to dryness, dissolved in chloroform containing diethylhexyl phtha-late as internal standard and chromatographed on an OV-17 stationary phase using flame ionisation detector. The results are compared with the BP method described for each formulation.     

UPLC-MS/MS method for the determination of acrylic acid in tap water

Abstract

A simple and rapid method employing ultra-high performance liquid chromatography tandem mass spectrometry has been developed for the direct determination of acrylic acid in tap water for the first time. The method worked on a ultra-high-performance liquid chromatography system and utilized the direct injection of 10?μL volumes. Aqueous samples were filtered with 0.22?μm membrane after diluting with the acetonitrile without any further pretreatment. The separation was accomplished by using a HILIC column with a gradient elution program. Acetonitrile and ammonium acetate solution (pH = 7) were applied in the method as the mobile phase. Acrylic acid- d₃ was used as the internal standard in the quantification process. The method provided good recovery from 102.8% to 104.4%, good precision with intraday relative standard deviations in a range of 2.3% and 5.1%. The limit of quantification for the method was 45?μg/L. The possible structures of qualitative ion and quantitative ion of acrylic acid were proposed in this work with the help of the product ion spectra of acrylic acid and its corresponding isotopic standards. This study provided a reliable and quantitative method that could be used for daily monitoring of water quality.     

HPLC Determination of Valproic Acid in Human Serum Using Ultraviolet Detection

Abstract

A sensitive HPLC method with minimal sample preparation and good reproducibility for the determination of valproic acid in serum is described. Serum samples were precipitated using acetonitrile containing diazepam as the internal standard. Chromatography was performed on a Hewlett Packard model 1090 equipped with an octadecylsilane column and a Beckman model 163 variable wavelength detector. The drug and internal standard were eluted isocratically using a mobile phase consisting of 0.01M sodium phosphate monobasic solution, pH 2.3 and acetonitrile (63:37 v/v) followed by a gradient to flush the column before the next sample injection. The flow rate was 2.5 mL/min, the injection volume was 25 μL and the effluent was monitored at 210 nm. The serum standard curve was linear from 2.5-200.0 μg/mL with a correlation coefficient of 0.9994. Day-to-day precision for quality control samples (10.0, 25.0, 75.0 μg/mL serum) ranged from 5.6-9.6% CV. Possible interferences from other drugs which might be administered concurrently were studied. The method has been applied to the analysis of human serum samples.     

Determination of Atenolol and Its Related Compounds by Ion Pair High Performance Liquid Chromatography

Abstract

A rapid, simple, accurate, and stability-indicating ion pair high performance liquid chromatography (IP HPLC) procedure is presented for the determination of atenolol in pharmaceutical tablets. The related compounds of atenolol were separated, making the determination specific for atenolol. An aliquot of the sample is dissolved in methanol containing N-butyryl-4-aminophenol as an internal standard and chromatographed on a supelcosil LC-8-DB (5μ) (25Omm × 4.6mm i.d.) column using 1.0 mM ammonium acetate and 2.0 mM octanesulfonic acid sodium salt in acetonitrile: water (25:75) solution adjusted to pH 3.5 with glacial acetic acid as the mobile phase. The detection was carried at 225 nm. The relative standard deviations are less than 1.0% for the two commercial products analyzed. The method was tested for linearity, recovery, and specificity.     

A New Simplified Microassay for the Quantitation of Theophylline in Serum by High-Performance Liquid Chromatography

Abstract

An improved, rapid and simplified HPLC method is presented for the quantitation of theophylline in serum. The internal standard, beta-hydroxypropyl theophylline (20 ul of a 100 ug/ml solution) is added to 50 ul of serum. Serum proteins are precipitated by the addition of 30 ul of 20% trichloroacetic acid solution. The mobile phase consists of a sodium acetate buffer with 8% acetonitrile. Chromatogram run time is 8 minutes. The sensitivity limit is 0.10 ug/ml. This method is interference free from the major metabolites of theophylline and other drugs commonly coadministered with theophylline.     

Assay of N-Propylajmaline in Blood Plasma by Ion-Pair Liquid-Liquid Chromatography

Abstract

A sensitive method for assay of N-propylajmaline (prajmaline) in human plasma is described. The quaternary ammonium compound exists as a pair of stereoisomers, which are isolated and separated by ion-pair liquid-liquid chromatography on microporous silica particles. An aqueous solution containing perchloric acid and sodium perchlorate is used as stationary phase and a mixture of butanol, dichloroethane and hexane as mobile phase. The procedure involves ion-pair extraction from plasma and evaporation prior to the chromatographic separation. Selective detection is achieved by using a fluorescence detector. The method allows assay of concentrations down to 10 pmol of the two forms of prajmaline in 1 ml of plasma with a relative standard deviation below 5 %.     

A Stability-Indicating Hplc Analysis of Famotidine and Its Application to Kinetic Studies

Abstract

A stability-indicating HPLC analytical method has been developed for the determination of the H₂-receptor antagonist, famotidine in the presence of its degradation products. the method utilizes reversed phase chromatography with UV detection and internal calibration techniques. the mobile phase was comprised of 84% ammonium acetate buffer (pH 2.9) and 16% acetonitrile and pumped at a flow rate of 1.5 ml/min. Quantitation was performed by measuring the peak height ratio of drug to internal standard (salicylic acid). the limit of famotidine detection was determined to be 10 ng (0.4 ug/ml) with a signal to noise ratio of 3:1. Within day coefficient of variation of the method was 2.22% (2.5 μg/ml) and 0.82% (10 μg/ml). Between day coefficient of variation based on the slopes of daily prepared standard curves was 4.70%. the developed method was used to determine the drug content of famotidine tablets. Further, it was used to investigate the kinetics of degradation of the drug in an acidic solution.     

High Performance Liquid Chromatographic Determination of Pirenzepine Dihydrochloride in Its Pharmaceutical Formulation

Abstract

A high-performance liquid chromatographic procedure for the determination of pirenzepine dihydrochloride as a bulk material and in its tablet dosage form (Gastrozepin^R) is presented. Normal phase liquid chromatography has been performed on a Micro-pack Si-10 column using ammonium hydroxide (28–30% NH₃) in methanol (0.75: 99.25% v/v) as mobile phase at a flow rate of 2 ml/min. Clobazam has been used as internal standard with retention times of 1.9 and 2.8 minutes for clobazam and pirenzepine dihydrochloride, respectively at 254 nm. Analytical calibration yields a linear relationship between 5 and 25 μg/ml, with correlation coefficient of 0.999. Tablets each labelled to contain 25 mg pirenzepine dihydrochloride give mean percentage found of 99.98 ± 0.4. A plot of logarithm of concentration against time for a solution in 6 N hydrochloric acid gives a straight line with a slope of - 0.197 day^?1. The proposed method is, therefore, a stability indicating method.     

Liquid Chromatographic Assay for Salicylic Acid in Liquid and Semisolid Formulations

Abstract

A high performance liquid chromatographic assay for quantitating salicylic acid (S) in lotion, collodion, ointment and cream formulations is described. The method involved direct determination of S in the liquid dosage forms after appropriate dilutions with the mobile phase. Prior extraction of S from ointments and creams was carried by chloroform. Metronidazole was used as the internal standard and a μ-Bondapak phenyl column with a mobile phase made of 30%, methanol in 5 mM solution of tetrabutylammonium phosphate (pH 7.5) led to an efficient separation. Retention times of about 3 and 7.5 min were obtained for the internal standard and S respectively. The recovery of S from the dosage forms was tested by adding known amounts of S to each preparation and mixing before determination. The mean percentage recovery was in the range of 98–101.1%. The method was found to be accurate, simple and reproducible.     

High Performance Liquid Chromatographic Determination of Testosterone Propionate,Progesterone and Estradiol Benzoate in Bovine Implants

Abstract

A Method for the determination of testosterone propionate, progesterone, and estradiol benzoate in bovine implants is presented. The method utilizes a Dupont, zorbax DDS analytical column with a mobile phase consisting of methanol, deionized water, and tetrahydrofuran (65:30:15 v/v). Sample preparation consists of of dissolution of the implant, followed by dilution and injection onto the HPLC system. The procedure is accurate, precise, linear, and specific for the implant steroids with quantitation by peak height, using dipenty 1 phthalate as the internal standard.     

Analysis of Thyroidal Amino Acids in Pharmaceutical Preparations. I - Reverse Phase High Pressure Liquid Chromatography Analysis of Sodium Liothyronine from Tablets

Abstract

A simple, sensitive and specific assay method was developed for the assay of sodium liothyronine (T₃Na) from tablets. Sodium liothyrorn'ne was extracted from powdered tablets with a solvent system consisting of butanol and dilute hydrochloric acid. The solvent was removed under vacuum and the residue was dissolved in ammonical methanol. An aliquot of this solution was injected on a μBondapak C₁₈ column and the elution was carried out with a mobile phase consisting of methanol:water:phosphoric acid (55:45: 0.1). The effluent was monitored by U. V. detection at 254 nm. A linear calibration curve was obtained in the range of 10 to 250 ng on column with a precision of ±4% (C. V.). The internal standard consisted of 3, 3′, 5-triiodothyronine (T3′ or RT₃). The usefulness of an alternate compound, 3, 5-diiodo-3′, 5′-dibromothyronine, which is not endogenous, was also demonstrated as an internal standard.     

Simultaneous determination of cyromazine,melamine and their biodegradation products by ion-pair high-performance liquid chromatography

An ion-pair high-performance liquid chromatography with ultraviolet detection method for the determination of cyromazine, melamine and its biodegradation products (ammeline, ammelide, cyanuric acid and biuret) was developed. C18 column was utilised to separate the six analytes with a mobile phase consisting of perchloric acid-ammonia solution and acetonitrile, under gradient elution and variable flow rate. The detection wavelengths were 205 nm for cyanuric acid and biuret and 222 nm for cyromazine, melamine, ammeline and ammelide. For analysis of sediment samples, the extraction solution containing acetonitrile, ammonia and water (80:10:10 by volume) was used to extract the analytes from sediment matrix. Using the extraction method for the spiked sediment sample, high linearity of matrix-matched standard curve could be obtained for the six analytes. The method detection limit was 0.1 μg g^?1 for melamine and cyromazine, 0.2 μg g^?1 for ammeline and ammelide, 1.2 μg g^?1 for cyanuric acid and 1.0 μg g^?1 for biuret in sediment matrix. The recoveries of these compounds were 70.1–98.3% and the relative standard deviations were 0.5–4.4%. Finally, the proposed method was successfully applied to the analysis of the sediment sample near the wastewater outlet of a melamine-producing factory.     

Determination of Propantheline Bromide in Tablet Formulations by Reverse-Phase HPLC

Abstract

The reported reverse-phase HPLC method for the determination of propantheline bromide, xanthanoic acid, xanthone, and 9-hydroxy-propantheline bromide in tablets is fast, sensitive, specific, accurate and reporoducible. Methyl xanthanoate is used as internal standard. The total elution time is 6 min. The method is stability-indicating since it can determine the degradation products. The column utilized was suplecosil LC-8 (5 micron), 250 mm × 4.6 mm i.d. The mobile phase was 0.03 M solution of ammonium acetate in acetonitrile: water: THF (60:38:2); the pH was adjusted to 4.5 with acetic acid, the detection was at 254 nm. A wavelength of 248 nm was used to quantitate xanthanoic acid and the flow rate was 1.5 mL/min. The proposed HPLC method was verified for linearity, accuracy, precision, and applicability.     

Development and validation of a UPLC–MS method for the determination of galantamine in guinea pig plasma and its application to a pre‐clinical bioavailability study of novel galantamine formulations

To evaluate the bioavailability and pharmacokinetic profiles of two novel galantamine formulations as medical countermeasure products, an ultra‐performance liquid chromatography–single quadrupole mass spectrometry (UPLC–MS) method was developed and validated for quantifying galantamine in guinea pig plasma using solid‐phase extraction with a mixed mode strong cation exchange reversed‐phase cartridge. Chromatographic separation was achieved on a Waters Acquity UPLC BEH C₁₈ column maintained at 40°C. The mobile phases were solution A, acetonitrile–water, 5:95 (v/v) and solution B, acetonitrile–water 90:10 (v/v), both containing 2 mM ammonium formate and 0.2% formic acid. The mobile phase was delivered utilizing a 3 min gradient program start with 95%A–5%B at a flow rate of 0.6 mL/min. The analyte and internal standard, galantamine‐d3, were detected by selected ion monitoring mode on a Waters 3100 single quadrupole mass spectrometer with positive electrospray ionization. The method was validated according to the US Food and Drug Administration bioanalytical guidance. The method was selective and was linear over the analytical range of 2–2000 ng/mL. Accuracy and precision were acceptable with intra‐ and inter‐day accuracies between 96.8 and 101% and precisions (RSD) <4.88%. The method was successfully implemented to measure galantamine plasma levels in a series of pre‐clinical bioavailability studies for the evaluation of novel galantamine formulations.     

Quantitation of Terbutaline Sulfate in Pharmaceutical Dosage Forms Using High Performance Liquid Chromatography

Abstract

A stability-indicating reverse phase high-performance liquid chromatography method has been developed to quantify terbutaline sulfate in pharmaceutical dosage forms. The method is accurate and precise with percent relative standard deviations based on 6 readings of 0.6 with an internal standard (salicylic acid) and 0.8 without an internal standard. The results are in excellent agreement with the USP-NF method. A decomposed sample gave 49.4% results with the developed method versus 71.3% with the USP-NF method.     

Use of Ethoxy-Homologs as Internal Standards for Determination of Urinary Vanillylmandelic Acid and Normetanephrine in Man by High Performance Liquid Chromatography

Abstract

Synthesis of the ethoxy-homologs of vanillylmandelic acid (3-ethoxy-4-hydroxymandelic acid, EMA) and normetanephrine (3-ethoxy-4-hydroxyphenylethanolamine, EHPEA) and their use in minor modifications of existing assays on human urine are described. For analysis of vanillylmandelic acid, the homologous internal standard is added to an aliquot of urine, organic acids are then extracted into ethyl acetate and back extracted into 10% K₂CO₃, and finally extracted a second time into ethyl acetate. After evaporation of the ethyl acetate, the residue is redissolved in the mobile phase to be used in the chromatography, and injected onto a reverse phase column. Comparison of results with a gas chromatography-mass spectrometry (GCMS) assay gave almost identical results (96% ± 2%, mean ± SE, n=10). Analysis of normetanephrine is performed by addition of internal standard to an aliquot of urine before heat hydrolysis of amine conjugates. The amines are adsorbed onto columns of Bio Rex 70, and then eluted with a solution of 1 M NH₄OH, which is then evaporated to dryness. After residue is redissolved in borate buffer, the amines are extracted into toluene:isoamyl alcohol and back extracted into 0.1 M acetic acid before injection onto a reverse phase column. Correlation with a GCMS assay gave similar results (102% ± 4%, mean ± SE, n=9).     

Simple Multiresidue Determination of Fluoroquinolones in Bovine Milk by Liquid Chromatography with Fluorescence Detection

Abstract

A simple and sensitive method for the simultaneous determination of five fluoroquinolones (ciprofloxacin, enrofloxacin, danofloxacin, difloxacin, and sarafloxacin) in bovine milk was developed. Protein precipitation from milk samples was achieved by the addition of acetonitrile and o‐phosphoric acid. Acetonitrile was removed with dichloromethane, leaving the fluoroquinolones in the acid aqueous extract. The aqueous extract was analyzed by liquid chromatography with fluorescence detection (LC–FD). The mobile phase was composed of acetonitrile and 10 mM citrate buffer solution of pH 4.5, with an initial composition of acetonitrile‐water (12∶88, v/v) and using linear gradient elution. Norfloxacin was used as an internal standard. The limits of detection found ranged from 1 to 6 ng · mL^?1 and were below the maximum residue limits (MRLs) established by the European Union. The proposed method was applied to the determination of these compounds in different bovine milk samples. Method validation was carried out by a recovery assay.     

An Ion Exchange Separation-Atomic Absorption Spectrophotometric Method for the Determination of Microgram Quantities of Copper,Iron and Zinc in Infant Milk Formula: Powder Form.

Abstract

An atomic absorption spectrophotometric method is described for the determination of microgram quantities of copper, iron and zinc in infant formula powdered milks. After sample digestion in concentrated nitric acid in a pressure vessel, the solution is evaporated till dryness, and then a solution of 6M HCl is added, in order to form the chlorocomplexes of the metals. This acid solution is passed through an ion-exchange column (anion exchange resin, chloride form). The metals are eluted from the column with diluted acid mixture of 0.005M HCl + 0.5% (v/v) HNO₃, and then the eluate is evaporated till dryness. The residue is dissolved in 1% (v/v) HNO₃, and then atomized into an air-acetylene flame. A standard addition procedure was employed as a back-up technique. The results obtained by this proposed method and those obtained by the standard addition technique were statistically treated, compared and discussed in this paper.     

Determination of Ergotamine Tartarate and Cyclizine Hydrochloride in Pharmaceutical Tablets by Reverse Phase HPLC

Abstract

A high performance liquid chromatographic procedure is presented for the determination of ergotamine tartarate and cyclizine hydrochloride in pharmaceutical tablets. An aliquot of the sample is dissolved in methanol containing ethyl p-hydroxybenzoate as an internal standard and chromatographed on a 5 üm, C₁₈, Hibar pre-packed, Lichrospher (250 mm × 4.0 mm i.d.), column using a mobile phase of 0.01 M ammonium acetate in acetonitrile: water: triethylamine (35:64:1) solution, the pH was adjusted to 3.7 with glacial acetic acid. The method was tested for linearity, recovery, and specificity and was found to be fast, sensitive, accurate and reproducible with a total elution time of six min.