High Pressure Liquid Chromatographic Assay for Salicylic Acid and its Metabolites in Rat Urine

Abstract

An HPLC method for the determination of salicylic acid (SA), gentisic acid (GA), salicyluric acid (SU), and salicyl acyl glucuronide (SAG) in rat urine was developed. The method consisted of extracting SA, GA, and SU from acidified urine into 50:50 mixture of ethyl acetate and butyl chloride. Salicyl acyl glucuronide was extracted from neutral urine after conversion to salicyl hydroxamic acid with hydroxylamine. Salicyl phenolic glucuronide was estimated indirectly as the difference between total salicylate and sum of the four constituents mentioned above. Chromatographic separation was done on a C₁₈ column with U.V. detection at 310 nm using a mobile phase consisting of 5–10% acetonitrile in 3% glacial acetic acid. The extraction recovery of these compounds from spiked urine ranged from 90–108%. The detection limits were 10 μg/ml for GA, SU and SA, and 2.5 μg/ml for SHA. The method was applied to the study of salicylic acid metabolism in the rat.     

Determination of Ascorbic Acid and Dehydroascorbic Acid in Blood Plasma Samples

Abstract

Following the stabilization of the plasma samples with HClO₄ and EDTA, the samples could be directly analyzed by HPLC using electrochemical detection and reversed-phase columns. The accuracy and precision of the method was evaluated using plasma samples spiked with ascorbic acid (10 μg/ml) and the results were also compared to the classical colorimetric procedure. Dehydroascorbic (5 μg/ml) was determined in plasma samples using UV detection following derivatization at room temperature for 45 minutes with o-phenylenediamine.     

Simultaneous Analysis of Pyridoxine and Melatonin in Tablet Formulation by Derivative Ultraviolet Spectroscopy

Abstract

A method for simultaneous analysis of pyridoxine and melatonin by second and third derivative UV - spectroscopy, the “zero - crossing” technique, is described. The determination has been carried out in 0.1 mol dm^?3 hydrochloric acid solution and the concentration range of 2 – 10 μg/ml pyridoxine and 0.5 – 3.5 μg/ml melatonin. Lower limits of detection at the 95% confidence level were 0.26 μg/ml for pyridoxine and 0.05μg/ml for melatonin The advantages of the proposed method include its application for the assay and in-vitro dissolution studies of pyridoxine and melatonin from two different tablet formulations.     

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.     

Determination of Arteether in Plasma Using a Simple and Rapid High-Performance Liquid Chromatographic Assay

Abstract

A simple and rapid high-performance liquid chromatographic (HPLC) assay for the determination of the antimalarial drug arteether in plasma was developed and validated in this report. Perchloric acid was used in this method as a plasma protein precipitant and to attain an acidic medium suitable for the decomposition of arteether to a derivative possessing UV absorption. This derivative and the internal standard (progesterone) were separated from the plasma on a 10 μm μ-Bondapack C₁₈ reversed-phase column at ambient temperature with a mobile phase composed of acetonitrile:water (60:40 v/v) and at a flow rate of 1.5 ml/min. The effluent was monitored at 254 nm with a UV detector. Linear relation between drug concentrations and peak height ratios of arteether derivative to the internal standard was achieved in the range of 0.25-10 μg/ml arteether with a detection limit of 50 ng/ml arteether in plasma. The within-day and between-days precisions were evaluated using 3 different concentrations of arteether. The values of the coefficients of variation were 1.35-1.68% and 1.65-2.82% for within-day and between-day, respectively. This method was applied to determine some pharmacokinetic parameters of arteether after intramuscular injection of 50 mg/kg arteether oily solution to rabbits.     

Preconcentration and Spectrophotometric Determination of Chromium (VI) and Total Chromium in Drinking Water by the Sorption of Chromium Diphenylcarbazone with Surfactant Coated Alumina

Abstract

A simple and inexpensive method for determining chromium (VI) in drinking water by spectrophotometry after preconcentration with sodium dodecyl sulphate (SDS) coated alumina column is described. Chromium(VI) is reacted with diphenylcarbazide (DPC) and the Cr-DPC complex is quantitatively adsorbed onto a SDS coated alumina column from 800 ml of sample solution. The complex is then eluted with a 8 ml mixture of methanol, acetone and hydrochloric acid and determined by spectrophotometry. Total chromium can be determined after oxidation of chromium (III) to chromium (VI) by KMnO₄. The relative standard deviation (10 replicate analyses) at the 10 μg l^?1 of chromium (VI) and 10 μg l^?1 of total chromium were 3.5% and 3.4% and corresponding limits of detection (based on 3 σ) were 0.040 μg l^?1 and 0.033 μg l^?1, respectively.     

Revised Method for Determination of Aspirin and Salicylic Acid in Human Plasma by High Pressure Liquid Chromatography

Abstract

The method for the analysis of aspirin and salicylic acid in human plasma has been updated to include advances in column technology, extraction procedures and absorbance detection. Aspirin and salicylic acid are extracted from acidified plasma into an organic solvent system containing internal standard. Following controlled evaporation under partial vacuum of the organic extract, the dried down-residue is reconstituted with mobile phase. Chromatography is ion suppression reverse phase on a 5 μm O.D.S. column with detection by absorbance at 237 nm and optional fluorescence. Concentration of aspirin as low as 0.20 μg/ml and salicyclic acid as low as 0.50 μg/ml can be quantitated.     

High Pressure Liquid Chromatographic Determination of Mecillinam in Human Plasma and Urine

Abstract

A simple, specific, rapid and sensitive method for the analysis of mecillinam in plasma and urine using high pressure liquid chromatography is described. The assay is performed by direct injection of a plasma protein free supernatant or a dilution of urine. A μBondapak phenyl column with an eluting solvent of 16% CH₃CN-0.2% H₃PO₄ was used, with UV detection of the effluent at 220 nm. Desacetyl-cephalothin was used as the internal standard and quantitation was based on peak height ratio of mecillinam to that of the internal standard. The lowest concentration detectable without extraction was 0.25 μg/ml for plasma and 8.9 μg/ml for urine. No interference from plasma and urine was noted.     

Absorption Spectra of 4f Electron Transitions of Neodymium and Erbium with 8-Hydroxyquinoline-5-sulphonic Acid and Diethylamine Systems and Its Analytical Application

Abstract

In this paper the absorption spectra of 4f electron transitions of the systems of neodymium and erbium with 8-hydroxyquino-line-5-sulphonic acid and diethylamine have been studied by normal and third-derivative spectrophotometry. Their molar absorptivities are 80 l.mol^?1.cm^?1 for neodymium and 65 l.mol^?1.cm^?1 for erbium. Use of the third-derivative spectra, eliminates the interference by other rare earths and increases the sensitivity for Nd and Er. The derivative molar absorptivities are 390 1.mol^?1.cm^?1 for Nd and 367 1.mol^?1.cm^?1 for Er. The calibration graphs were linear up to 11.8 μg/ml of Nd and 12.3 μg/ml of Er, respectively. The relative standard deviations evaluated from eleven independent determinations of 7.2 μg/ml (for Nd) and 8.3 μg/ml (for Er) are 1.3% and 1.4%, respectively. The detection limits (signal to noise ratio = 2) are 0.2 μg/ml for Nd and 0.3 μg/ml for Er. The method has been developed for determining those two elements in mixture of lanthanides by means of the third-derivative spectra and the analytical results obtained are satisfactory.     

A Fluorimetric Method for the Determination of Cyanide with Fluorescein and Iodine∗

Abstract

A rapid, simple and sensitive fluorimetric method has been developed for the determination of cyanide with fluorescein as fluorogenic reagent (λ_ex = 494 nm, λ_em = 514 nm) at pH 6.0–7.0. A linear calibration curve was obtained in the range 0.004–2.0 μg CN^?/25 ml. The detection limit is 0.004 μg CN^-/25 ml. The method was successfully applied to the determination of cyanide in waste water.

     

Reversed‐phase liquid chromatography with electrospray mass detection and 1H and 13C NMR characterization of new process‐related impurities,including forced degradants of Efavirenz: Related substances correlated to the synthetic pathway

In this study, a stability‐indicating reversed‐phase liquid chromatographic electrospray mass spectrometric method was developed and validated for the determination of process‐related impurities and forced degradants of Efavirenz in bulk drugs. Efavirenz was subjected to acid, alkaline hydrolysis, H₂O₂ oxidation, photolysis, and thermal stress. Significant degradation was observed during alkaline hydrolysis, and the degradants were isolated on a mass‐based purification system and characterized by high‐resolution mass spectrometry, positive electrospray ionization tandem mass spectrometry, and ¹H and ¹³C NMR spectroscopy. Accurate mass measurement and NMR spectroscopy revealed the possible structure of process‐related impurities and degradant under stress conditions. The acceptable separation was accomplished on Waters bondapak C₁₈ column (250 mm × 4.6 mm; 5 μm), using 5 mM ammonium acetate and acetonitrile as a mobile phase in a gradient elution mode at a flow rate of 1.0 mL/min. The eluents were monitored by diode array detector at 247 nm and quantitation limits were obtained in the range of 0.1–2.5 μg/mL for Efavirenz, degradants, and process‐related impurities. The liquid chromatography method was validated with respect to accuracy, precision, linearity, robustness, and limits of detection and quantification as per International Conference on Harmonization guidelines.     

Colorimetric Determination of Propofol in Bulk form,Dosage Form and Biological Fluids

ABSTRACT

Propofol is coupled with 2, 6-dichloroquinone-4-chlorimide (DCQ) in a reaction buffered at pH 9.6 to give a colored product having an analytically useful maximum at 635 nm. The factors affecting the color generation were optimized and incorporated in the procedure. The reacted propofol has a molar absorptivity of 3.9 × 10^?4 L mol^?1 cm^?1, and Beer's law is obeyed for concentrations 1-5 μg ml^?1 with detection limit 0.25 μg ml^?1. The method was found applicable to biological fluids (plasma and urine) spiked with propofol at concentration levels 1-5 μg ml^?1 for plasma and 1-5 μg 0.5 ml^?1 urine (less sensitivity is obtained with urine volumes above 0.5 ml) with detection limits 0.28 μg ml^?1 for plasma and 0.4 μg 0.5 ml^?1 urine. The average recovery for the commercial preparation (1% w/v propofol emulsion intravenous injection for infusion) was 99.54% with an RSD of 1.05%. The method was validated by an adopted HPLC method. The results obtained by the HPLC method for the commercial preparation were statistically compared with the proposed method and evaluated at the 95% confidence limits.     

Kinetic Flow Injection Spectrophotometric Determination of Nitrite by its Catalytic Effect on the Oxidation of Chlorophosphonazo-pN by Bromate

Abstract

A flow injection kinetic method has been developed for the determination of nitrite, based on its catalytic effect on bromate oxidation of chlorophosphonazo-pN in H₂SO₄ medium. The reaction is followed spectrophotometrically by measuring the decrease in the absorbance at 551 nm. The sampling frequency was 83 h^?1. The calibration curve was linear between 0.050 and 1.00 μg/ml, and the detection limit was 0.018 μg/ml. The proposed method was applied to the determination of nitrite in waters and soil with satisfactory results.     

Determination of Formaldehyde in Waste Water by Lucigenin Chemilummescence

Abstract

A chemiluminescence analysis has been developed for the determination of formaldehyde based on its inhibition of the chemiluminescence reaction of lucigenin-C10^?-H₂o₂. The method is sensitive, convenient and selective with a detection limit of 0.05ng/ml. The linear dynamic range is 1.0ng/ml to 0.1 μg/ml. The variation coefficient of ten determinations for 2.Ong/ml formaldehyde is 1.2%. Applications to the trace determination of formaldehyde in industrial waste waters are discussed.     

Simultaneous Determination of Tinidazole and Furazolidone in Suspension by HPTLC and HPLC

Abstract

High performance thin layer chromatographic (HPTLC) and high performance liquid chromatographic (HPLC) methods were developed for the simultaneous determination of Tinidazole and Furazolidone in suspension.

In the HPTLC method the separation of Tinidazole and Furazolidone was carried out on silica gel 60F₂₅₄ HPTLC glass plate using chloroform:methanol:ammonia (9:1:0.1 v/v) as a mobile phase. Rf values obtained were 0.63 and 0.79 for Furazolidone and Tinidazole respectively. Densitometric evaluation was done at 335 nm. Linearity was obtained within the concentration range 10–50 μg/ml and 3.5–17.5 μg/ml for Tinidazole and Furazolidone respectively.

The second method is based on high performance liquid chromatography on a reversed phase column (μ Bondapak C₁₈) using a mobile phase comprised of water: acetonitrile: triethylamine (80:20:0.1 v/v) adjusted to pH = 3.0 with dil. phosphoric acid. Retention times were 5.24 and 7.82 min for Tinidazole and Furazolidone respectively at a flow rate of 1.5 ml/min. Detection was done at 335 nm. Linearity was obtained within the concentration range 30–180 μg/ml and 10.5–63 μg/ml for Tinidazole and Furazolidone resp.     

High Pressure Liquid Chromatography Assay for Determination of 18-β-Glycyrrhetinic Acid in Plasma

Abstract

This report presents a useful high pressure chromatography assay for determination of the proposed chemopreventive agent 18-β-glycerrhetinic acid (GA) in murine and human plasma. Drug was released from plasma proteins through precipitation with a mixture of sodium bisulfate and sodium chloride after which it was extracted with acetonitrile. Standard calibration curves of GA covered the concentration range of 2.5 to 120 μg/ml. The lower limit of detection was 0.5 μg/ml. No endogenous plasma constituents from plasma were found to interfere with the determination of GA. Recover of GA from plasma was greater than 95% over a concentration range of 20 to 100 μg/ml. Linearity of the assay was excellent; within-run precision showed a C.V. of 4.2% at 25 μg/ml, 5.6% at 20 μg/ml and 3.4% at 120 μg/ml. Between-run assay precision and accuracy was also considered to be excellent. The specificity, sensitivity and reproducibility of the procedure are adequate for proposed clinical pharmacology studies of this agent.     

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.     

A Fluorescence Quenching Method for the Determination of Iodide Ion with Salicylfluorone and Hydrogen Peroxide

Abstract

A highly sensitive and selective fluorescence quenching method has been developed for rapid determination of iodide ion with salicylfluorone (SAF) as fluorogenic reagent (λ_ex = 495 nm, λ_em = 520 nm) at pH 2.5-3.0. The calibration graph is linear over the range 0.05-300 μg/25 ml. The detection limit is 0.05 μ/25 ml iodide. Other halide ions do not interfere with the determination even when present in large excess. The method is rapid and was successfully applied for the determination of iodide ion in sodium chloride, table salt and low sodium salt.     

A Fluorescence Quenching Method for the Determination of Bromate Ion with 4,5-Dibromophenylfluorone and Cetyltrimethylammonium Bromide

Abstract

A highly sensitive and selective fluorescence quenching method was developed to determine the bromate ion (BrO₃ ^?) with 4,5-dibromophenylfluorone (DB-PF) as fluorogenic reagent. BrO₃ ^? reacts with potassium bromide in sulfuric acid solution (0.6M) giving bromine (Br₂) which is estimated with fluorescence quenching method using DB-PF as fluorogenic reagent. Bromine reacts with DB-PF to produce a compound, whose maximum excitation wavelength and emission wavelength are 543nm, 560nm respectively. The linear calibration range is 0.05–0.5 μg/25ml. The detection limit is 0.05μg/25ml. The method may be used to determine microamounts of BrO₃ ^? in potassium chlorate with satisfactory results. The method offers the advantages of simplicity, rapidity and sensitivity.     

Spectrophotometric Determination of Trimethoprim in Pure Form and in Pharmaceutical Preparations using Bromothymol Blue,Bromocresol Green and Alizarin Red S

ABSTRACT

Simple, sensitive and selective methods for the determination of trimethoprim (TMP) in pure form and in pharmaceutical formulations are described. The methods are based on the reaction of TMP as a π-electron donor with bromothymol blue (BTB), bromocresol green (BCG) and alizarin red S (ARS) as electron acceptors. The coloured products are quantified spectrophotometrically at their corresponding λ_max.

Beer's law is obeyed in case of BTB in the range 2.9-23.2 μg/ml (CHCl₃), 2.9-20.0 μg/ml (CH₂Cl₂) and 5.0-29.0 μg/ml (ClC₆H₅), in the case of BCG 2.9-27.5 μg/ml (H₂O/alc.), 2.9-18.3 μg/ml (CHCl₃) and 2.9-20.3 μg/ml (CH₂Cl₂) and for ARS in the range 3.0-12.0 μg/ml in H₂O/alc medium.

The specific absorptivities, molar absorptivities, Sandell sensitivities, standard deviations and percent recoveries are evaluated. Application of the suggested methods to dosage forms is presented and compared with the pharmacopoeial method. The interference from additives and sulfa compounds, especially sulfamethoxazole, has been overcome by extraction into chloroform or methylene chloride.