Determination of piribedil in pharmaceutical formulations by micellar electrokinetic capillary chromatography

A fast and simple micellar electrokinetic capillary chromatographic method was developed for the analysis of piribedil in pharmaceutical formulations. The effects of buffer concentration, buffer pH, sodium dodecyl sulphate (SDS) concentration, organic modifier, applied voltage and injection time were investigated. Optimum results were obtained with a 50 mM borate buffer at pH 8.0 containing 50 mM SDS by using a fused silica capillary (50 m internal diameter, 72 cm effective length). The sample was injected hydrodynamically for 4 s at 50 mbar pressure and the applied voltage was +30 kV. The detection wavelength was set at 205 nm. Diflunisal was used as an internal standard. The analysis was performed at 25 °C and the total run time was 14 min. The method was suitably validated with respect to linearity range, limit of detection and quantification, precision, accuracy, specificity and robustness. The linear calibration range was 5–100 g mL^–1 and the limit of detection was determined as 1 g mL^–1. The method developed was successfully applied to the determination of piribedil in pharmaceutical formulations. The results were compared with a spectrophotometric method reported in the literature and no significant difference was found statistically.     

Determination of flurbiprofen in pharmaceutical formulations by UV spectrophotometry and liquid chromatography

In this study, a new and rapid UV spectrophotometric (UV) method and a reversed phase high performance liquid chromatographic (LC) method were developed for quantitative estimation of flurbiprofen, a non-selective, non-steroidal, anti-inflammatory drug (NSAID), in pure form and in pharmaceutical dosage form. The solvent system, wavelength of detection, chromatographic conditions were optimized in order to maximize the sensitivity of both the proposed methods. The linear regression equations obtained by least square regression method were Abs=7.5906×10⁻² concentration (μg/ml) + (−) 4.6210×10⁻² for the UV method, and peak area=1.2652×10² concentration (ng/ml) + 1.4830×10³ for the LC method. The detection limit as per the error propagation theory was found to be 0.34 μg/ml for UV method and 15 ng/ml for LC method. The developed methods were successfully employed with high degree of precision and accuracy for the estimation of total drug content in two commercial ophthalmic drops of flurbiprofen. The results of analysis were treated statistically, as per USP 2000 and International Conference on Harmonization (ICH) guidelines for validation of analytical procedures, and by recovery studies. The results obtained from UV method were comparable with those obtained by using LC. It was concluded that both the developed methods are equally accurate, sensitive, precise, reproducible, robust and rugged and could be applied directly and easily to the pharmaceutical preparations of flurbiprofen. However, LC method is useful at very low level (ng/ml), whereas UV method is suitable at μg/ml level.     

Determination of adsorption by fluorescence in gas chromatography

PMBF₂, a pyrromethene pigment, can be used in gas chromatography. Because of its fluorescence, adsorption sites on glass columns and connections can be traced in situ. The compound can be employed to check the inertness of glass surfaces after deactivation procedures. Some applications are described.     

Determination of mono and disaccharide content of enteral formulations by gas chromatography

Summary A quantitative GC method has been developed which allows determination of mono and disaccharides in enteral formulations. The method is based on the isolation of the mono and disaccharide fraction on a charcoal-celite column and conversion to trimethylsilylated oximes (TMS-oximes). The repeatability of the complete method and recovery were acceptable. In the five commercial samples assayed, maltose was the main sugar (5.24–8.85 gL⁻¹) followed by glucose (1.06–2.41 gL⁻¹) and lactose (0–1.17 gL⁻¹) Low levels of fructose (0–0.18 gL⁻¹) and sucrose (0–0.07 gL⁻¹) were observed and galactose was detected in two of the samples. The presence of maltulose is reported in enteral formulations for the first time. Maltulose formed from maltose during processing, was present in variable amounts (0.12–1.07 gL⁻¹) and could be a useful indicator for enteral formulation classification.     

气相色谱/质谱测定水产品中氯霉素残留量

样品经均质后,用乙酸乙酯提取,正己烷脱脂,C18小柱净化,衍生后用GC ECD,NCI GC MS,NCI GC MSMS多种方法定性及定量测定,外标法定量。在0.1μg/kg水平,回收率为72%～110%,平行测定9次后相对标准偏差为16 5%。质量浓度在0～10μg/L范围内呈良好线性关系,相关系数r=0.9997。     

Determination of midazolam and its major hydroxy metabolite in plasma by gas liquid chromatography. Application to a pharmacokinetic study

A sensitive gas liquid chromatographic (GLC) assay was developed for plasma determinations of 8-chloro-6-(2′ -fluorophenyl)-1-methyl-4H-imidazo[1,5 α][1,4]benzodiazepine (compound I) and its hydroxymethylimidazo metabolite (compound II). The internal standards used were 8-chloro-6-(2′ -chlorophenyl)-1 -methyl-4H-imidazo[1,5 α][1,4]benzodiazepine (compound VI) and 7-chloro-5-(2′ -fluorophenyl)-1, 3-dihydro-1-(hydroxyethyl)-2H-1,4-benzodiazepin-2-one (compound VII) for compounds I and II, respectively. Following extraction, and silylation for compound II, compounds I and II were analyzed by GLC using a glass column packed with 5% OV-101 on Gas-Chrom Q, and a ⁶³Ni electron-capture detector. The GLC method was validated by a CI-GC/MS technique. The detection limit of the assay is approximately 4–5 ng/ml for compound I and 3 ng/ml for compound II. The method was used in comparative pharmacokinetic studies of the distribution of the two compounds in arterial and venous blood.     

Determination of fluoxetine, fluvoxamine, and clomipramine in pharmaceutical formulations by capillary gas chromatography

A simple and fast capillary gas chromatographic method with flame ionization detection is proposed for the simultaneous determination of fluoxetine, fluvoxamine, and clomipramine without a prederivatization. The reported method is the first one that allows the determination of three selective serotonin reuptake inhibitors. Optimal conditions for the quantitative separation were investigated: column head pressure (80 kPa), injector and detector temperatures (260 and 250 degrees C), time and temperature for the splitless step (0.75 min and 60 degrees C), size of sample (2 microL), and oven temperature program, providing analysis times shorter than 10 min. Aspects such as the stability of the solutions, linearity, accuracy, and precision are examined in order to validate this method. Peak purity and detection and quantitation limits are also assessed using mass selective detection. The scope of the validated method is tested in the analysis of pharmaceutical preparations, with recoveries between 97.5 and 102.5% with regard to their nominal contents.     

The application of chromatography to the analysis of pharmaceutical creams

Summary The application of GLC, HPLC and TLC to the analysis of pharmaceutical creams is discussed with special attention to sample clean-up. The results of the determination of hydrocortisone acetate, salicylic acid, benzoic acid, diethyl stilbestrol, chloramphenicol, diphenhydramine HCl, tretinoin and some cream base components by reversed phase HPLC are given.Presented at the 14th International Symposium on Chromatography London, September, 1982     

Determination of phenolic antioxidants in pharmaceutical formulations by liquid chromatography and migration study on HDPE packagings

Summary The performance of UV diode-array, spectrometric and electrochemical detectors was compared in the chromatographic analysis of trace amounts of six phenolic antioxidants. Quantitative validation was undertaken; the linearity range was wider using UV detection although the limits of detection were lower with electrochemical detection. UV detection was applied both to identification of an antioxidant in a hydrophilic suspension and to a migration study.     

Determination of streptomycin in pharmaceutical preparations by gas chromatography

The antibiotic streptomycin can be reliably quantitated in injectable pharmaceuticals by GC. The manipulations are not difficult, and total analysis time for duplicate samples is less than twenty minutes. Reaction of the drug with aqueous sodium hydroxide solution generates maltol, which is extracted into chloroform prior to silylation. The silyl ether of maltol is then assayed, using naphthalene as internal standard. Duplicate analyses of twenty pharmaceutical samples showed a relative standard deviation of ±1.3%.     

Room-temperature,phosphorimetric determination of the beta-blocking agent pindolol in pharmaceutical tablets,urine and blood serum

It is already recognised that heavy-atom-induced, room-temperature phosphorescence can be used to determine pindolol in pharmaceutical samples and biological fluids. We describe here a new, simple, rapid and selective development of this technique. The phosphorescence signals derive from the interaction of pindolol with a relatively high concentration of heavy-atom salts in the presence of sodium sulphite as oxygen scavenger. Phosphorescence was registered in the presence of 1.2 M potassium iodide, 15 mM sodium sulphite and 30% v/v methanol at 450 nm, exciting at 285 nm. The detection limit was 21.1 ng mL⁻¹. The method has been successfully applied to the determination of pindolol in commercial pharmaceutical tablets, urine and blood serum.     

Determination of tropicamide in pharmaceutical formulations using high-performance liquid chromatography

An isocratic, reversed-phase liquid chromatographic method was developed for determination of tropicamide using atropine as an internal standard in a pharmaceutical dosage form. Tropicamide and atropine sulfate were separated using a microBondapak ODS (C18) column by isocratic elution of mobile phase with flow rate of 2.0 ml/min. The mobile phase composition was methanol-50 mM phosphate buffer (pH 4; 30:70, v/v). The eluate was monitored at 257 nm with detector range setting fixed at 0.01 AUFS. Under these conditions, the retention times were 4.81 min for atropine and 11.89 min for tropicamide. The standard calibration curve was linear over a sample concentration range from 2 to 300 microg/ml, with limit of detection of 0.15 microg/ml. The assay linearity was good (typically r2 = 0.9992) and the standard curves were linear in the detection range. The precision of the method (expressed by relative standard deviation) and the accuracy (mean error in percent) were <5% for both intra- and inter-day assays. Recovery at 80-120% of labeled claim ranged from 98.4 to 100.7% for tropicamide. The proposed method was satisfactorily applied to the determination of tropicamide in pharmaceutical preparation and stability indicating studies.     

离子对分离和抑制电导检测法测定四乙基铵和四丁基铵根离子

建立了季铵盐的离子色谱分析方法.采用Dionex DX-500 型离子色谱仪,C18柱,电导检测器,以30%乙腈和10 mmol/L甲烷磺酸混合溶液为流动相,流量为1.00 mL/min.四乙基溴化铵和四丁基溴化铵的质量浓度和峰面积的相关系数分别为0.9996和0.9994;线性范围分别为10～80 mg/L和20～120 mg/L;检出限分别为0.28和0.76 mg/L;RSD分别为1.3%、 2.5%.该方法可用于分析水溶液中季铵盐的含量.     

气相色谱法测定饼干类食品中氯丙醇类化合物

报道了饼干类食品中3-氯-1,2．丙二醇和1,3-二氯-2-丙醇的测定。采用乙醚索氏提取、甲醇萃取净化,再经N,O-双（三甲基硅烷）三氟乙酰胺（BSTFA）衍生,毛细管气相色谱法分离,FID作检测器。方法检出限为0．01mg／kg,回收率在90％～105％,相对标准偏差为2．2％～9．3％,     

反相离子对色谱法测定间苯二磺酸钠

运用反相高效离子对色谱法测定了间苯二磺酸钠.采用C18色谱柱(250 mm×4.6 mm i.d.,5 μm),流动相为V(乙腈):V(50 mmol/L NaH2PO4)＝7:93(含0.05%四丁基氢氧化铵),流速为1.0 mL/min,检测波长210 nm,柱温:30 ℃.间苯二磺酸钠在0.32×10-3～81.92×10-3 mg/mL范围内线性关系良好,r＝0.9999,加样回收率为98.8%～101.1%,RSD＝0.73%(n＝7).本法为工业生产间苯二磺酸钠提供了分析方法.