Electrochemical Detection of Retinoids Using Normal Phase HPLC

Abstract

Non-aqueous electrochemical (EC) detection of 13-cis-retinoic acid, all-trans retinoic, acitretin and vitamin A palmitate in non-aqueous solvents are reported.

Non-aqueous (EC) detection allows for normal-phase chromato-graphy of these compounds prior to detection. The normal phase system used a mobile phase of HEX/THF/AcOH for the separation of all four compounds. The stationary phase was either silica or PVA-sil. The lipophilic salts, t-butylammoniumtetrafluoroborate or t-butyl-ammoniumhexafluorophosphate necessary for EC detection were added post-column.

The limit of detection (LOD) for EC detection of these compounds is approximately 1 ng on column compared with an LOD by UV absorption of 2 ng on column.

The linear detection for these compounds with the EC detector was about two orders of magnitude.     

Ion Exchanger Liquid Chromatography of N-Acetylaspartic Acid and Some N-Acetylaspartyl Peptides

Abstract

A high performance liquid chromatographic (HPLC) procedure for the rapid separation of N-acetylaspartic acid, N-acetyl-aspartyl-glutamic acid and N-acetylaspartyl-glutamyl-aspartic acid is described. The procedure utilizes a pellicular ion-exchange column support, and ionic strength gradient with mobile phase solutions buffered to pH 5.0 and a UV detector operated at 210 nm. Reproducibility and quantitative capabilities are also discussed. The method has been used for a tentative estimation of N-acetylaspartic acid and N-acetylaspartyl peptides in a rat brain synaptosomal extract.     

The Preparative Scale Reverse Phase HPLC Separation of Epimeric Alkaloids Using Camphorsulfonic Acid as an Ion Pairing Reagent

Abstract

A reverse phase paired ion HPLC procedure is described for the separation of multigram quantities of epimeric alkaloids using camphorsulfonic acid as the ion-pairing reagent.     

Studies on the Synthesis and Antiproliferative Activities of 13‐cis‐Retinoyl Sugar Derivatives

New retinoyl sugar derivatives of 13‐cis‐retinoic acid were synthesized in three ways in this paper in order to enhance pharmacal effects, especially antiproliferative activities of 13‐cis‐retinoic acid. Their structures were confirmed by IR, ¹H‐NMR, ¹³C‐NMR, and MS spectra and their antiproliferative activities were determined in vitro using human cancer lines. Results showed that some compounds possessed potential antitumor activities.     

High Performance Liquid Chromatographic Assay of Hydromorphone Hydrochloride Injection

Abstract

A stability indicating high performance liquid chromatographic (HPLC) method for determining hydromorphone hydrochloride in dosage forms is described. The drug was chromatographed on a C₁₈ reverse phase column, using a mobile phase consisting of sodium lauryl sulfate, acetic acid, acetonitrile and water, and detected at 280 nm. Linearity of detector response to the concentration was confirmed. The procedure showed excellent reproducibility and gave quantitative recoveries of the drug from spiked placebos. Photodegraded samples of the dosage form, were assayed by the HPLC procedure and the current USP spectrophotometric procedure. Comparison of the results showed that the USP procedure is only partially stability indicating.     

Rapid Analysis of 6-Diazo-5-oxo-L-norleucine (DON) in Human Plasma and Urine

Abstract

A paired-ion, reversed phase high pressure liquid chromatography (HPLC) procedure is described for the analysis of DON in human plasma and urine. Plasma proteins are removed by centrifugal membrane filtration, and the filtrate is injected directly onto an octadecylsilane column. The DON is eluted in a mobile phase consisting of 5 mM 1-heptanesulfonic acid, pH 2.4. Eluting material is monitored at 280 nm and 254 nm. The lower limit of sensitivity in plasma is 0.1 μg/ml.     

Determination of Phthalic Anhydride In Workplace Air Using Reverse Phase High Performance Liquid Chromatography

Abstract

A reverse phase high performance liquid chromatographic procedure is described for the analysis of phthalic anhydride in workplace air. A glass fibre filter was used to collect the airborne phthalic anhydride and the analyte was then desorbed and hydrolyzed with dilute aqueous sodium hydroxide. Subsequent acidification of this solution with the mobile phase enabled the phthalic anhydride to be determined as phthalic acid using UV detection.     

An HPLC Method for the Determination of Theophylline and Its Metabolites in Serum and Urine

Abstract

A urine and a serum assay have been developed to quantitate theophylline and its major metabolites:1,3-dimethyluric acid, 3-methylxanthine and 1-methyluric acid. Reverse phase chromatography follows a serum acetone extraction procedure and a urine anion exchange clean-up procedure. Lower limits of sensitivity are 0.04 μg/ml for serum metabolites and 1 μg/ml for urine metabolites. Both assays are free of interference from endogenous substances. These assays have been tested successfully in pharmacokinetic and metabolic studies of theophylline.     

Paired-Ion High Pressure Liquid Chromatography of Methotrexate and Metabolites in Biological Fluids

Abstract

A paired-ion high pressure liquid chromatography procedure (HPLC) is described for the separation of methotrexate and its major metabolites (7-hydroxymethotrexate, 4-amino-4-deoxy-N^lO-methylpteroic acid, methotrexate diglutamate, methotrexate triglutamate), and therapy-related compounds (Diamox and 5-methyltetrahydrofolate). The mobile phase consisted of a 70% solution of 5 mM hexanesulfonic acid, pH 3.75, and 30% methanol eluted on a reverse phase column or columns and monitored at 305 nm or 280 nm UV absorption. The lower limit of sensitivity for methotrexate and 7-hydroxymethotrexate in plasma was 2 ng/ml.     

Liquid Chromatographic Resolution of Enantiomers on Chiral Amide Bonded-Silica Gel Normal Phase Separation of Racemic α-Amino Acid Derivatives by N-Acetyl-L-valyl-aminopropyl-silanized Silica (AVA) Phase

Abstract

A new optically active stationary phase obtained by grafting N-acetyl-L-valine with 3-aminopropylsilanized silica was developed. The high-efficiency chiral column was prepared by slurry packing procedure. Direct resolution of the racemates of α-amino acid derivatives was accomplished by using normal phase liquid chromatography.     

Simultaneous Analysis Of Estradiol Dienanthate,Estradiol 3-Benzoate And Testosterone Enanthate Benzilic Acid Hydrazone In Oily Formulations Bygradient-Hplc

Abstract

A procedure is described for the analysis of estradiol-3-benzoate, testosterone enanthate benzylic acid hydrazone and estradiol dienanthate in oily solution. The multi-step gradient reversed phase ion-pairing HPLC method uses 1-pentane sulfonic acid sodium salt (0.0025 M in 0.1% acetic acid methanolic solution): acetonitrile and water (55 : 30 to 45 : 15 to 0) mobile phase gradient and a 250 × 4.6 mm, 5 micron octadecyl silane column, with 1,2,4,5-tetrachlorobenzene as internal standard. The time required for chromatography is 31 minutes. The method gives relative standard deviations (RSD) of .94% or better for the assay of active ingredients in commercial formulations.     

Simultaneous Determination of Phenylpropanolamine Hydrochloride and Isopropamide in Capsule∗ by High Performance Liquid Chromatography Using CROWNPAK Column

Abstract

A procedure is described for the assay of phenylpropanolamine hydrochloride & isopropamide by HPLC using CROWNPAK column and detection at 200 nm. The system was aqueous perchloric acid as mobile phase containing 5 % methanol. Linearity studies were carried out using peak height measurements. There was > 99 % recovery and coefficient of variation was < 2% for formulation. The procedure was rapid, accurate, precise and specific for the assay of phenylpropanolamine HCl in presence of isopropamide.     

Liquid Anion Exchange Studies and Separation of Mercury

Abstract

A new method is developed for the extractive separation of mercury from associated elements. Mercury is quantitatively extracted from 0.5 M acetic acid solution by aliquat 336 S, which acts as a liquid anion exchanger. The metal ion from the organic phase is stripped with sodium hydroxide solution and determined in the aqueous phase complexometrically. The extracted species is [2(R₄N⁺), Hg(OAc)₄ ^?2]. A working procedure for the selective separation of mercury from zinc, cadmium, nickel, cobalt, copper, bismuth and manganese is described.     

High-Performance Liquid Chromatography of Domoic Acid,a Marine Neurotoxin,with Application to Shellfish and Plankton

Abstract

A recent outbreak of poisoning resulting from the consumption of cultured blue mussels (Mytilus edulis L.) from a localized area in Eastern Canada has been attributed to the presence of domoic acid (1), a relatively rare neurotoxic amino acid, previously found only in some algae of the family Rhodomelaceae. Studies on aqueous extracts of shellfish tissue indicated that the toxin and several of its isomers could be separated (and isolated in sufficient amounts for subsequent structural identification) by reversed-phase high-performance liquid chromatography (HPLC) with ultraviolet (UV) diode array detection (DAD). Aqueous acetonitrile containing 0.1% v/v trifluoroacetic acid was used as mobile phase. As the retention time and characteristic UV absorption spectrum of 1 (λ_max = 242 nm) permit unequivocal identification, the HPLC-DAD procedure was refined with a microbore column to provide a rapid (5 min), sensitive (0.3 ng detection limit) and reproducible assay method for the determination of 1 in shellfish tissue. Extraction was accomplished by boiling homogenized shellfish tissue for 5 min with distilled water. Extracts were taken through an octadecylsilica solid phase extraction clean-up prior to HPLC. This method has been applied to a variety of shellfish and phytoplankton samples.

BRIEF

Reversed-phase HPLC with ultraviolet diode array detection was used to analyze shellfish tissue and phytoplankton extracts for domoic acid. A rapid (5 min) and sensitive (0.3 ng detection limit) assay is presented.     

Determination of Bendroflumethiazide in Plasma by High Performance Liquid Chromatography and Fluorescence Detection

Abstract

An accurate, precise, and specific assay is described for the determination of bendroflumethiazide (BFTZ) in plasma. The procedure employs a C18 column, a mobile phase consisting of 35% acetonitrile in 0.015M phosphoric acid, and a fluorescence detector with a 254nm excitation filter and a 400nm emission filter. Furosemide is used as the internal standard. Using lml of plasma, this method can detect 10ng/ml of BFTZ.     

Reverse Phase HPLC For Rapid,Comprehensive Measurement of Nucleotides,Nucleosides and Bases of The Myocardial Adenine Pool

Abstract

A novel reverse phase HPLC method is described for the simultaneous measurement of adenosine tri-, di- and monophosphates (ATP, ADP, AMP), inosine monophosphate (IMP), adenosine, inosine, hypoxanthine, nicotinamide adenine dinucleotide (NAD) and uric acid in cardiac tissues and coronary effluent. The use of a simplified perchloric acid extraction procedure and ODS columns easily modified with Mq⁺⁺, Tris and phosphate buffer, allows considerable saving in analysis time together with extremely good resolution, particularly for ATP and ADP, and provides a very practical tool for the routine assessment of changes in adenine pool metabolites.     

Ion Chromatographic Determination of Sodium Isethionate

Abstract

Single column anion chromatography with conductivity detection has been used for the determination of sodium isethionate. A mobile phase of aqueous phthalic acid - methanol (pH 2.5) allows for the separation of isethionate from chloride and alkyl isethionate ester surfactants. Commercially available samples of sodium isethionate and alkyl esters were analyzed by the described procedure.     

Quantitation of Glipizide and Glyburide in Tablets Using High Performance Liquid Chromatography

Abstract

Reverse phase high-performance liquid chromatography methods for the quantitation of glipizide and glyburide in tablets have been developed. The methods are accurate and precise with a percent relative standard deviations based on 6 injections of 0.8 and 0.3% for glipizide and glyburide, respectively. The developed methods can be used to test the content uniformity of the tablets. The extraction procedure for the active ingredients from the tablets is very simple. There is no interference from the excipients and the acid hydrolyzed samples showed new peak in the chromatograms.     

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 %.     

Ion Chromatographic Determination of Dibutylphosphoric Acid in Nuclear Fuel Reprocessing Streams

Abstract

A rapid method has been developed for the determination of dibutylphosphoric acid (DBP), a degradation product of tributylphosphate (TBP), which is used in a solvent extraction process for recovery of uranium. DBP along with any monobutylphosphoric acid (MBP) and phosphoric acid are extracted from the organic phase into dilute sodium hydroxide. DBP is separated from MBP and phosphoric acid by ion chromatography and is determined on a peak height ratio basis. The method requires only 30 minutes per analysis as compared to the conventional alumina column separation-colorimetric determination procedure which requires 8 h to complete. DBP has been quantified to a lower limit of 1.5 mg/L. Relative standard deviations ranging from 5.7% to 0.4% were obtained for DBP concentrations ranging from 1.5 to 500 mg/L, respectively.