Your search keyword '"Antitussive Agents analysis"' showing total 139 results

51. Spectrophotometric determination of some anti-tussive and anti-spasmodic drugs through ion-pair complex formation with thiocyanate and cobalt(II) or molybdenum(V).

Author

El-Shiekh R, Zahran F, and El-Fetouh Gouda AA

Subjects

1-Butanol chemistry, Antitussive Agents isolation & purification, Drug Stability, Hydrogen-Ion Concentration, Parasympatholytics isolation & purification, Pharmaceutical Preparations chemistry, Reproducibility of Results, Solvents, Spectrophotometry, Ultraviolet, Antitussive Agents analysis, Cobalt chemistry, Molybdenum chemistry, Parasympatholytics analysis, Thiocyanates chemistry

Abstract

Two rapid, simple and sensitive extractive specrophotometric methods has been developed for the determination of anti-tussive drugs, e.g., dextromethorphan hydrobromide (DEX) and pipazethate hydrochloride (PiCl) and anti-spasmodic drugs, e.g., drotaverine hydrochloride (DvCl) and trimebutine maleate (TM) in bulk and in their pharmaceutical formulations. The proposed methods depend upon the reaction of cobalt(II)-thiocyanate (method A) and molybdenum(V)-thiocyanate ions (method B) with the cited drugs to form stable ion-pair complexes which extractable with an n-butnol-dichloromethane solvent mixture (3.5:6.5) and methylene chloride for methods A and B, respectively. The blue and orange red color complexes are determined either colorimetrically at lambdamax 625 nm (using method A) and 467 or 470 nm for (DEX and PiCl) or (DvCl and TM), respectively (using method B). The concentration range is 20-400 and 2.5-50 microg mL-1 for methods A and B, respectively. The proposed method was successfully applied for the determination of the studied drugs in pure and in pharmaceutical formulations applying the standard additions technique and the results obtained in good agreement well with those obtained by the official method.

Published

2007

52. Possible role of pseudoephedrine and other over-the-counter cold medications in the deaths of very young children.

Author

Wingert WE, Mundy LA, Collins GL, and Chmara ES

Subjects

Acetaminophen analysis, Adolescent, Analgesics, Non-Narcotic analysis, Antitussive Agents analysis, Brompheniramine analysis, Central Nervous System Depressants analysis, Child, Child, Preschool, Chlorpheniramine analysis, Databases as Topic, Dextromethorphan analysis, Doxylamine analysis, Ethanol analysis, Female, Forensic Toxicology, Gas Chromatography-Mass Spectrometry, Histamine H1 Antagonists analysis, Humans, Infant, Male, Philadelphia, Pyridines analysis, Bronchodilator Agents analysis, Cause of Death, Common Cold drug therapy, Ephedrine analysis, Nonprescription Drugs adverse effects

Abstract

The Philadelphia Medical Examiners Office has reported a series of 15 deaths between February 1999 and June 2005 of infants and toddlers 16 months and younger in which drugs commonly found in over-the-counter (OTC) cold medications were present. A total of 10 different drugs were detected: pseudoephedrine, dextromethorphan, acetaminophen, brompheniramine, carbinoxamine, chlorpheniramine, ethanol, doxylamine and the anticonvulsants, phenobarbital, and phenytoin. The drugs were confirmed and quantified by gas chromatography (GC)-mass spectrometry, with the exception of ethanol, which was analyzed by headspace GC and of phenobarbital and phenytoin that were quantified by GC with a nitrogen phosphorus detector. The most predominant drug was pseudoephedrine, which was found in all of the cases (blood concentration, n=14, range=0.10-17.0 mg/L, mean=3.34 mg/L) and was the sole drug detected in three cases. Acetaminophen was detected in blood from each of the five cases with sufficient sample. Other drugs (with frequency of detection) were dextromethorphan (five cases), carbinoxamine (four cases), chlorpheniramine (two cases) and brompheniramine, doxylamine, and ethanol (one case each). In the majority of the cases, toxicity from drugs found in easily available OTC medications was listed either as the direct cause of death or as a contributory factor. The manner of death was determined to be natural in only two of the cases. This postmortem study supports previous evidence that the administration of OTC cold medications to infants may, under some circumstances, be an unsafe practice and in some cases may even be fatal. The treating physicians and the general public need to be made more aware of the dangers of using OTC cold medications to treat very young children so that these types of tragedies might be avoided.

Published

2007

53. A new hydrophilic interaction liquid chromatographic (HILIC) procedure for the simultaneous determination of pseudoephedrine hydrochloride (PSH), diphenhydramine hydrochloride (DPH) and dextromethorphan hydrobromide (DXH) in cough-cold formulations.

Author

Ali MS, Ghori M, Rafiuddin S, and Khatri AR

Subjects

Acetates chemistry, Buffers, Chemical Phenomena, Chemistry, Physical, Chromatography, High Pressure Liquid, Drug Combinations, Hydrogen-Ion Concentration, Indicators and Reagents, Pharmaceutical Solutions, Reference Standards, Reproducibility of Results, Solvents, Spectrophotometry, Ultraviolet, Antitussive Agents analysis, Dextromethorphan analysis, Diphenhydramine analysis, Ephedrine analysis, Histamine H1 Antagonists analysis, Nasal Decongestants analysis

Abstract

A new HILIC method has been developed for the simultaneous determination of pseudoephedrine hydrochloride (PSH), diphenhydramine hydrochloride (DPH) and dextromethorphan hydrobromide (DXH) in cough-cold syrup. Mobile phase consists of methanol:water (containing 6.0 g of ammonium acetate and 10 mL of triethylamine per liter, pH adjusted to 5.2 with orthophosphoric acid), 95:5 (v/v). Column containing porous silica particles (Supelcosil LC-Si, 25 cm x 4.6 mm, 5 microm) is used as stationary phase. Detection is carried out using a variable wavelength UV-vis detector at 254 nm for PSH and DPH, and at 280 nm for DXH. Solutions are injected into the chromatograph under isocratic condition at constant flow rate of 1.2 mL/min. Linearity range and percent recoveries for PSH, DPH and DXH were 150-600, 62.5-250, 75-300 microg/mL and 100.7%, 100.1% and 100.8%, respectively. Method is stability indicating and excipients like saccharin sodium, sodium citrate, flavour and sodium benzoate did not interfere in the analysis. Compounds elute in order of increasing ionization degree caused by cation-exchange mechanism in a run time of less than 15 min. Mobile phase pH is manipulated to regulate ionization and ion-exchange interaction and thereby retention of compounds.

Published

2007

54. [Wavelength interval selection by iteratively reinitialized GA and its application to spectrophotometric determination of components in cough syrup].

Author

Cheng B, Wu XH, and Chen DZ

Subjects

Algorithms, Antitussive Agents analysis, Spectrophotometry

Abstract

Wavelength selection in PLS calibration can be used to reach two goals: improve the predictive ability and simplify the model. Iteratively reinitialized GA is a modified genetic algorithm, and it gives an initializing procedure of selecting the first candidates for every run of GA, which uses the results of previous runs as the guiding information. This algorithm can select wavelength regions instead of scattering points, which is very helpful in understanding the relevant parts of spectra. Furthermore, the continuous wavelength points make the PLS model more robust. Appling IRGA based wavelength selection to the UV-Vis spectrum of cough syrup, the result illustrates that PLS regression can greatly benefit from variable selection when used for multicomponent spectrophotometric determination.

Published

2006

55. Development of a rapid multi-element method of analysis of antitussive syrups by inductively coupled plasma atomic emission spectrometry and direct sample introduction.

Author

Zachariadis GA and Kapsimali DC

Subjects

Antitussive Agents analysis, Metals analysis, Spectrophotometry, Atomic methods

Abstract

A new rapid method was developed and optimized for routine multi-element determination of traces of metals in antitussive syrups using direct introduction of diluted syrup into the nebulization system of inductively coupled plasma atomic emission spectrometer (ICP-AES). Using a Scott-type double-pass spray chamber combined with a cross-flow nebulizer, the optimum ICP conditions, like RF incident power, argon gas flow rate and nebulizer sample uptake flow rate were found. A critical objective of the study was to evaluate the matrix effect on the intensity and consequently on the sensitivity of the developed method. Thus, the maximum syrup concentration which could be introduced into the argon plasma, was estimated. The sensitivity variation was calculated as compared to the corresponding sensitivity obtained from aqueous solutions for each analyte. The performance characteristics of the proposed method were evaluated for quantitative and semi-quantitative determination and finally, the method was applied to the analysis of various commercial antitussives.

Published

2006

56. Application and validation of chemometrics-assisted spectrophotometry and liquid chromatography for the simultaneous determination of six-component pharmaceuticals.

Author

El-Gindy A, Emara S, and Mostafa A

Subjects

Antitussive Agents analysis, Diphenhydramine analysis, Expectorants analysis, Guaifenesin analysis, Least-Squares Analysis, Parabens analysis, Preservatives, Pharmaceutical analysis, Principal Component Analysis, Reproducibility of Results, Sodium Benzoate analysis, Technology, Pharmaceutical, Theophylline analysis, Bronchodilator Agents chemistry, Chromatography, High Pressure Liquid methods, Complex Mixtures chemistry, Spectrophotometry, Ultraviolet methods

Abstract

Three methods are developed for the simultaneous determination of theophylline anhydrous (TH), guaiphenesin (GP), diphenhydramine hydrochloride (DP), methylparaben (MP), propylparaben (PP) and sodium benzoate (BZ) in pharmaceutical syrup. The chromatographic method depends on a high performance liquid chromatographic separation on a reversed-phase C(18) column at ambient temperature with mobile phase consisting of 25 mM KH2PO4, pH 3.2-acetonitrile (60:40, v/v). Quantitation was achieved with UV detection at 222 nm based on peak area. The other two chemometric methods applied were partial least squares (PLS-1) and principal component regression (PCR). These approaches were successfully applied to quantify the six components in the studied mixture using information included in the UV absorption spectra of appropriate solutions in the wavelength range of 220-270 nm with Deltalambda=0.4 nm. The calibration PLS-1 and PCR models were evaluated by internal validation (prediction of compounds in its own designed training set of calibration), by cross-validation (obtaining statistical parameters that show the efficiency for a calibration fit model) and by external validation over synthetic and pharmaceutical preparation. The results of PLS-1 and PCR methods were compared with the HPLC method and a good agreement was found.

Published

2006

57. Liquid chromatography and chemometric-assisted spectrophotometric methods for the analysis of two multicomponent mixtures containing cough suppressant drugs.

Author

El-Gindy A, Emara S, Mesbah MK, and Hadad GM

Subjects

Acetonitriles analysis, Acetonitriles pharmacology, Benzoic Acid analysis, Buffers, Calibration, Chemistry, Pharmaceutical methods, Chlorpheniramine analysis, Dextromethorphan analysis, Ephedrine analysis, Hydrogen-Ion Concentration, Ions, Parabens analysis, Phenylephrine analysis, Principal Component Analysis, Regression Analysis, Reproducibility of Results, Salts analysis, Sodium analysis, Sodium Benzoate analysis, Software, Sulfonic Acids analysis, Technology, Pharmaceutical instrumentation, Technology, Pharmaceutical methods, Ultraviolet Rays, Antitussive Agents analysis, Chromatography, Liquid methods, Spectrophotometry methods

Abstract

Three methods were applied for the analysis of 2 multicomponent mixtures containing dextromethorphan hydrobromide, phenylephrine hydrochloride, chlorpheniramine maleate, methylparaben, and propylparaben, together with either sodium benzoate (Mix 1) or ephedrine hydrochloride and benzoic acid (Mix 2). In the first method, liquid chromatography was used for their simultaneous determination using an ODS column with a mobile phase consisting of acetonitrile-phosphate buffer, pH 2.7 (40 + 60, v/v), containing 5mM heptanesulfonic acid sodium salt and ultraviolet (UV) detection at 214 nm. Also, 2 chemometric methods, principal component regression, and partial least squares were used. For both chemometric calibrations, a concentration set of the mixture consisting of each compound in each mixture was prepared in distilled water. The absorbance data in the UV spectra were measured for the 76 or 71 wavelength points in the spectral region 210-240 or 210-224 nm considering the intervals of deltagamma = 0.4 or 0.2 nm for Mix 1 and Mix 2, respectively. The 2 chemometric methods did not require any separation step. These methods were successfully applied for the analysis of the 2 multicomponent combinations in synthetic mixtures and in commercial syrups, and the results were compared with each other.

Published

2005

58. Simultaneous determination of some active ingredients in cough and cold preparations by gas chromatography, and method validation.

Author

Harsono T, Yuwono M, and Indrayanto G

Subjects

Acetaminophen analysis, Acetates analysis, Analysis of Variance, Caffeine analysis, Chlorpheniramine analysis, Dextromethorphan analysis, Drug Combinations, Electrophoresis, Capillary instrumentation, Electrophoresis, Capillary methods, Ephedrine analysis, Guaifenesin analysis, Nasal Decongestants analysis, Phenylpropanolamine analysis, Reproducibility of Results, Software, Temperature, Time Factors, Ultrasonics, Antitussive Agents analysis, Chemistry, Pharmaceutical methods, Chromatography, Gas methods, Expectorants analysis, Technology, Pharmaceutical methods

Abstract

A simple and rapid gas chromatographic (GC) method has been developed for the simultaneous determination of combinations of acetaminophen, phenylpropanolamine hydrochloride, guaifenesin, pseudoephedrine hydrochloride, caffeine, chlorpheniramine maleate, and dextromethorphan hydrobromide in cough and cold tablets and syrups. After extraction of the analyte with alkaline ethyl acetate, 2 microL extract was injected (splitting ratio of 50:1) into a gas chromatograph equipped with a CBP1-M25-025 fused silica capillary column (25 m x 0.22 mm; film thickness, 0.25 microm). The column temperature was held at 150 degrees C for 5 min, increased to 175 degrees C at 3 degrees C/min, and increased to 270 degreesC at 10 degrees C/min. The temperatures of the flame ionization detector and injector were maintained at 300 degrees C. The GC method is inexpensive, rapid, accurate, and precise, and thus it can be used for routine analysis of tablet and syrup preparations in quality control laboratories of pharmaceutical companies.

Published

2005

59. Simultaneous spectrophotometric determination of salbutamol and bromhexine in tablets.

Author

Habib IH, Hassouna ME, and Zaki GA

Subjects

Algorithms, Chromatography, High Pressure Liquid, Pharmaceutical Preparations analysis, Regression Analysis, Spectrophotometry, Ultraviolet methods, Tablets chemistry, Albuterol analysis, Antitussive Agents analysis, Bromhexine analysis

Abstract

Typical anti-mucolytic drugs called salbutamol hydrochloride and bromhexine sulfate encountered in tablets were determined simultaneously either by using linear regression at zero-crossing wavelengths of the first derivation of UV-spectra or by application of multiple linear partial least squares regression method. The results obtained by the two proposed mathematical methods were compared with those obtained by the HPLC technique.

Published

2005

60. On-line solid phase extraction using the Prospekt-2 coupled with a liquid chromatography/tandem mass spectrometer for the determination of dextromethorphan, dextrorphan and guaifenesin in human plasma.

Author

Kuhlenbeck DL, Eichold TH, Hoke SH 2nd, Baker TR, Mensen R, and Wehmeyer KR

Subjects

Antitussive Agents analysis, Humans, Spectrometry, Mass, Electrospray Ionization instrumentation, Chromatography, High Pressure Liquid, Dextromethorphan blood, Dextrorphan blood, Expectorants analysis, Guaifenesin analysis, Spectrometry, Mass, Electrospray Ionization methods

Abstract

An on-line liquid chromatography/tandem mass spectrometry (LC-MS/MS) procedure, using the Prospekt- 2 system, was developed and used for the determination of the levels of the active ingredients of cough/cold medications in human plasma matrix. The experimental configuration allows direct plasma injection by performing on- line solid phase extraction (SPE) on small cartridge columns prior to elution of the analyte(s) onto the analytical column and subsequent MS/MS detection. The quantitative analysis of three analytes with differing polarities, dextromethorphan (DEX), dextrorphan (DET) and guaifenesin (GG) in human plasma presented a significant challenge. Using stable-isotope-labeled internal standards for each analyte, the Prospekt-2 on-line methodology was evaluated for sensitivity, suppression, accuracy, precision, linearity, analyst time, analysis time, cost, carryover and ease of use. The lower limit of quantitation for the on-line SPE procedure for DEX, DET and GG was 0.05, 0.05 and 5.0 ng mL(-1), respectively, using a 0.1 mL sample volume. The linear range for DEX and DET was 0.05-50 ng mL(-1) and was 5-5,000 ng mL(-1) for GG. Accuracy and precision data for five different levels of QC samples were collected over three separate days. Accuracy ranged from 90% to 112% for all three analytes, while the precision, as measured by the %RSD, ranged from 1.5% to 16.0%

Published

2005

61. Development and validation of a capillary electrophoresis method for the determination of codeine, diphenhydramine, ephedrine and noscapine in pharmaceuticals.

Author

Gomez MR, Sombra L, Olsina RA, Martínez LD, and Silva MF

Subjects

Hydrogen-Ion Concentration, Reproducibility of Results, Antitussive Agents analysis, Codeine analysis, Diphenhydramine analysis, Electrophoresis, Capillary methods, Ephedrine analysis, Noscapine analysis

Abstract

The present work describes a simple, accurate and rapid method for the separation and simultaneous determination of codeine, diphenhydramine, ephedrine and noscapine present in cough-cold syrup formulations by capillary zone electrophoresis. Factors affecting the separation were the buffer pH and concentration, applied voltage, and presence of additives. Separations were carried out in less than 10 min with a 20 mM sodium tetraborate buffer, pH 8.50. The carrier electrolyte gave baseline separation with good resolution, great reproducibility and accuracy. Calibration plots were linear over at least three orders of magnitude of analyte concentrations, the lower limits of detection being within the range 0.42-1.33 microg ml(-1). Detection was performed by UV absorbance at wavelengths of 205 and 250 nm. Quantification of the components in actual syrup formulations was calculated against the responses of freshly prepared external standard solutions. The method was validated and met all analysis requirements of quality assurance and quality control. The procedure was fast and reliable and commercial pharmaceuticals could be analyzed without prior sample clean-up procedure.

Published

2005

62. Single-point plasma or urine dextromethorphan method for determining CYP3A activity.

Author

Kuo BP, Hu OY, Hsiong CH, Pao LH, Chen TS, and Hung CF

Subjects

Administration, Oral, Adult, Antitussive Agents blood, Antitussive Agents urine, Area Under Curve, Chromatography, High Pressure Liquid, Cytochrome P-450 CYP3A, Delayed-Action Preparations, Dextromethorphan blood, Dextromethorphan metabolism, Dextromethorphan urine, Humans, Male, Metabolic Clearance Rate, Phenotype, Saliva metabolism, Antitussive Agents analysis, Aryl Hydrocarbon Hydroxylases metabolism, Dextromethorphan analogs & derivatives, Dextromethorphan analysis, Oxidoreductases, N-Demethylating metabolism

Abstract

Dextromethorphan is used widely in vivo to phenotype the polymorphically expressed cytochrome P450 (CYP) 2D6. Also dextromethorphan is N-demethylated in vivo to 3-methoxymorphinan by human CYP3A4/5. The metabolic ratio (MR) of dextromethorphan/3-methoxymorphinan in plasma, saliva and urinary were examined as a possible in vivo probe of CYP3A activity. In limited previous studies, 4 h urinary samples were collected for determining the MR. To evaluate the repeatability and validity of previously reported and other potential phenotyping methods, the MR from urine samples (at various intervals), from plasma and from saliva (at varying time points) were determined after repetitive single doses of immediate-release or repetitive multiple doses of controlled-release dextromethorphan preparations. For the single-dose study, each of 12 subjects received 15 mg of immediate-release dextromethorphan in periods II and I, respectively, with a 1 week washout period. For the multiple dose study, each of 16 subjects received 60 mg controlled release dextromethorphan twice daily for 5 days in periods I and II, respectively, with a 2 week washout period. Dextromethorphan and 3-methoxymorphinan are assayed by high-performance liquid chromatography. In the single-dose study, all of the urine MR revealed good repeatabilities for the periods (paired t-test). The urine MR at any time interval of 0-6 h, 0-8 h and 0-12 h correlated significantly with the MR from 0-24 h urine (r>0.8, p<0.05). In the multiple-dose study, all MR revealed good repeatabilities for the two periods (paired t-test). The plasma MR at any time between 0.5 h and 12 h, the saliva MR at 12 h and the urine MR at any interval between 0-2 h, 0-4 h, 0-6 h, 0-8 h, 0-12 h and 0-24 h could predict the MR from AUCtau(ss). In conclusion, the urine sample as 0-6 h, 0-8 h or 0-12 h in the single immediate-release dose (15 mg) or in the multiple controlled-release dose (60 mg) procedure, the saliva sample at 12 h, the urine sample at 0-2 h, 0-4 h, 0-6 h, 0-8 h, 0-12 h, 0-24 h or all plasma-sampling points 0.5-12 h could be used as the dextromethorphan MR for determining the CYP3A activity., (Copyright 2003 John Wiley & Sons, Ltd.)

Published

2003

63. HPLC determination of aminophylline, methoxyphenamine hydrochloride, noscapine and chlorphenamine maleate in compound dosage forms with an aqueous-organic mobile phase.

Author

Yin C, Tang C, and Wu X

Subjects

Capsules, Chromatography, High Pressure Liquid, Drug Combinations, Indicators and Reagents, Reference Standards, Reproducibility of Results, Solutions, Spectrophotometry, Ultraviolet, Adrenergic beta-Agonists analysis, Aminophylline analysis, Antitussive Agents analysis, Bronchodilator Agents analysis, Chlorpheniramine analysis, Methamphetamine analogs & derivatives, Methamphetamine analysis, Noscapine analysis

Abstract

A high-performance liquid chromatography procedure for the simultaneous determination of aminophylline, methoxyphenamine hydrochloride, noscapine and chlorphenamine maleate in commercially available compound capsule dosage forms has been developed and validated. The separation and quantification were achieved on an Ultrasphere C18 column using a mobile phase of dichloromethane-methanol-0.25% (v/v) diethylamine aqueous solution (20:60:20, v/v/v) at a flow rate of 1 ml min(-1) with detection of all analytes at 264 nm. The separation was achieved within 6 min for each drug mixture. The method showed good linearity for the aminophylline, noscapine, chlorphenamine maleate and methoxyphenamine hydrochloride mixture in the 125-750, 35-210, 10-60 and 62.5-375 microg ml(-1) ranges, respectively. The intra- and inter-day R.S.D.s ranged from 0.4 to 0.5%, 0.4-0.6%, 0.5-0.7% and 0.4-0.6% for aminophylline, noscapine, chlorphenamine maleate and methoxyphenamine hydrochloride, respectively. The recoveries (mean+/-S.D.) of low, middle and high concentrations were 99.9+/-0.9, 100.4+/-1.3 and 99.7+/-0.7% for aminophylline; 99.9+/-1.1, 100.4+/-0.7 and 100.1+/-0.8% for noscapine; 99.8+/-1.1, 99.7+/-1.0 and 100.7+/-0.8% for chlorphenamine maleate; and 99.8+/-0.9, 100.4+/-1.6 and 99.9+/-0.9% for methoxyphenamine hydrochloride, respectively.

Published

2003

64. Sustained modelling ability of artificial neural networks in the analysis of two pharmaceuticals (dextropropoxyphene and dipyrone) present in unequal concentrations.

Author

Cámara MS, Ferroni FM, De Zan M, and Goicoechea HC

Subjects

Anti-Inflammatory Agents, Non-Steroidal analysis, Antitussive Agents analysis, Computer Simulation, Electrochemistry, Molecular Structure, Nonlinear Dynamics, Pharmaceutical Preparations chemistry, Dextropropoxyphene analysis, Dipyrone analysis, Neural Networks, Computer, Pharmaceutical Preparations analysis

Abstract

An improvement is presented on the simultaneous determination of two active ingredients present in unequal concentrations in injections. The analysis was carried out with spectrophotometric data and non-linear multivariate calibration methods, in particular artificial neural networks (ANNs). The presence of non-linearities caused by the major analyte concentrations which deviate from Beer's law was confirmed by plotting actual vs. predicted concentrations, and observing curvatures in the residuals for the estimated concentrations with linear methods. Mixtures of dextropropoxyphene and dipyrone have been analysed by using linear and non-linear partial least-squares (PLS and NPLSs) and ANNs. Notwithstanding the high degree of spectral overlap and the occurrence of non-linearities, rapid and simultaneous analysis has been achieved, with reasonably good accuracy and precision. A commercial sample was analysed by using the present methodology, and the obtained results show reasonably good agreement with those obtained by using high-performance liquid chromatography (HPLC) and a UV-spectrophotometric comparative methods.

Published

2003

65. Impurity profiling of pholcodine by liquid chromatography electrospray ionization mass spectrometry (LC-ESI-MS).

Author

Denk OM, Skellern GG, and Watson DG

Subjects

Antitussive Agents chemistry, Chromatography, High Pressure Liquid, Chromatography, Liquid, Codeine chemistry, Drug Contamination, Morpholines chemistry, Antitussive Agents analysis, Codeine analogs & derivatives, Codeine analysis, Morpholines analysis, Spectrometry, Mass, Electrospray Ionization methods

Abstract

Previously, a dimorpholinoethyl pholcodine manufacturing impurity was reported to be present in some samples of pholcodine. Apart from this impurity and morphine, other unknown impurities were detected in all the samples analysed by HPLC and micellar electrokinetic capillary chromatography. In this study, liquid chromatography mass spectrometry (LC-MS) analysis of samples of pholcodine showed that two of the previously unidentified compounds had mass spectra with molecular ions which differed from pholcodine by 16 amu. From this observation and other experimental data it was concluded that they are hydroxy derivatives of pholcodine. 10-S-hydroxy-pholcodine, which was synthesized by the oxidation of pholcodine with chromic acid, had the same chromatographic properties as one of these compounds. An early eluting compound in the LC-MS chromatograms of pholcodine was identified as pholcodine-N-oxide by matching chromatographic and mass spectral data of a synthesized pholcodine-N-oxide standard. The reaction of pholcodine with m-chloroperoxybenzoic acid not only produced the mono N-oxide, but also pholcodine-di-N,N'-oxide.

Published

2002

66. AAS and AES determination of furaltadone, methadone and trazodone in pharmaceutical formulations.

Author

Khalil S and El-Ries MA

Subjects

Anti-Infective Agents, Urinary analysis, Antitussive Agents analysis, Cadmium Compounds, Chemistry, Pharmaceutical, Reproducibility of Results, Selective Serotonin Reuptake Inhibitors analysis, Solutions, Spectrophotometry, Atomic, Zinc Compounds, Methadone analysis, Nitrofurans analysis, Oxazolidinones analysis, Trazodone analysis

Abstract

Ion-associate complexes of furaltadone, methadone and trazodone hydrochlorides with [Cd(SCN)(4)](2-) and [Zn(SCN)(4)](2-) were precipitated and the excess unreacted cadmium or zinc complex was determined. A new method using atomic emission and atomic absorption spectrometry for the determination of the above drugs in pure solutions and in pharmaceutical preparations is given. The drugs can be determined by the affort method in the ranges 7.2-72.16, 6.9-69.18 and 8.1-81.6 microg/ml solutions of the three drugs, respectively.

Published

2002

67. [Quantitative determinations of glycyrrhizic acid, glycyrrhetinic acid, morphine and sodium benzoate in compound liquorice tablets by capillary zone electrophoresis].

Author

Sun GX, Wang Y, and Sun YQ

Subjects

Antitussive Agents analysis, Drug Compounding, Electrophoresis, Capillary methods, Expectorants analysis, Glycyrrhetinic Acid analysis, Tablets, Glycyrrhizic Acid analysis, Morphine analysis, Sodium Benzoate analysis

Abstract

Capillary zone electrophoresis (CZE) was used to quantitatively determine the contents of glycyrrhizic acid, glycyrrhetinic acid, morphine and sodium benzoate in compound liquorice tablets. The detection wavelength was 228 nm and the applied voltage was 14 kV. Borax solution of 50 mmol/L was used as the background electrolyte and hydrochlorothiazide as the internal standard. There were all good linear relationships between the concentrations and the relative areas of glycyrrhizic acid, glycyrrhetinic acid, morphine and sodium benzoate. Their average recoveries were 98.2%, 97.3%, 97.1% and 97.5%, respectively. The method is simple, rapid and accurate.

Published

2002

68. A non-potentiometric sensing method for the determination of pentoxyverine with PQC sensors based on ion-pair complexes.

Author

Yuan J, Hu Y, Nie L, and Yao S

Subjects

Quartz, Antitussive Agents analysis, Chemistry Techniques, Analytical methods, Cyclopentanes analysis

Abstract

The construction and general performance characteristics of three piezoelectric quartz crystal sensors responsive to the pentoxyverine are described here. This kind of non-potentiometric sensing method is based on use of ion-pair complexes of the pentoxyverine cation with three counter anions, namely, tungstophosphate, tetraphenylborate and picrolonate. The complexes were embedded in a PVC matrix. Adsorption of the pentoxyverine ion on the complex caused a frequency decrease of the crystal. The frequency decrease was proportional to the amount of adsorbed analyte. The influencing factors were investigated in detail, and then optimized. The proposed sensors exhibit reasonable selectivity and a higher sensitivity than the potentiometric sensors. For a sensor modified with pentoxyverine-phosphotungstate, the calibration graph was linear over concentration of 1.0 x 10(-7) - 5.0 x 10(-5) M with a detection limit of 6 x 10(-8) M at pH 5.4.

Published

2001

69. A fast and efficient determination of amines and preservatives in cough and cold liquid and suspension formulations using a single isocratic ion-pairing high performance [correction of power] liquid chromatography method.

Author

Paciolla MD, Jansen SA, Martellucci SA, and Osei AA

Subjects

Chemistry, Pharmaceutical, Reproducibility of Results, Amines analysis, Antitussive Agents analysis, Chromatography, High Pressure Liquid methods, Nasal Decongestants analysis, Preservatives, Pharmaceutical analysis

Abstract

A single, highly selective ion-pairing reverse phase-high power liquid chromatography (RP-HPLC) method has been developed for the determination of amines and preservatives in a wide range of Tylenol((R)) liquid and suspension liquid products. As with many OTC products, the challenge is to quantitatively extract the analytes from difficult matrices and specifically analyze them in the presence of various excipients and flavors. Historically, separate analytical methods were used for each class of analytes (acids, bases and neutral compounds). In this method a mobile phase consisting of a buffered ion-pairing agent with acetonitrile, methanol and tetrahydrofuran was used to separate the charged amines from neutral and acidic compounds on a Phenomenex LUNA C8(2) 75 x 4.6 mm i.d. analytical column with a 3-microm particle size. The analytes include acids (benzoic acid), bases (pseudoephedrine, chlorpheniramine, dextromethorphan, doxylamine and diphenhydramine) and a neutral compound (butylparaben). The effects of pH, the chain length of the ion-pairing reagent, ionic strength and organic modifiers on the separation are discussed. The method is linear from 15 to 150% of the target amounts. The optimized method proves to be specific, robust and accurate for the analysis of the compounds.

Published

2001

70. HPLC determination of guaifenesin with selected medications on underivatized silica with an aqueous-organic mobile phase.

Author

Wilcox ML and Stewart JT

Subjects

Antitussive Agents analysis, Bronchodilator Agents analysis, Capsules, Chromatography, High Pressure Liquid, Codeine analysis, Dextromethorphan analysis, Drug Combinations, Ephedrine analysis, Indicators and Reagents, Reference Standards, Reproducibility of Results, Silicon Dioxide, Solutions, Expectorants analysis, Guaifenesin analysis

Abstract

A high performance liquid chromatography procedure has been developed for the simultaneous determination of guaifenesin pseudoephedrine-dextromethorphan and guaifenesin-pseudoephedrine in commercially available capsule dosage forms and guaifenesin-codeine in a commercial cough syrup dosage form. The separation and quantitation are achieved on a 25-cm underivatized silica column using a mobile phase of 60:40%) v/v 6.25 mM phosphate buffer, pH 3.0 - acetonitrile at a flow rate of 1 ml min(-1) with detection of all analytes at 216 nm. The separation is achieved within 10 min for each drug mixture. The method showed linearity for the guaifenesin-pseudoephedrine-dextromethorphan mixture in the 50-200, 7.5-30 and 2.5-10, microg ml(-1) ranges, respectively. The intra- and inter-day RSDs ranged from 0.23 to 4.20%, 0.18 to 2.85%, and 0.13 to 5.04% for guaifenesin, pseudoephedrine, and dextromethorphan, respectively. The guaifenesin pseudoephedrine mixture yielded linear ranges of 25-100 and 3.75-15 microg ml(-1) and intra- and inter-day RSDs ranged from 0.65 to 4.18% and 0.23 to 3.00% for guaifenesin and pseudoephedrine, respectively. The method showed linearity for the guaifenesin-codeine mixture in the 25-100 and 2.5-10 microg ml(-1) ranges and RSDs ranged from 0.37 to 4.25% and 0.14 to 2.08% for guaifenesin and codeine, respectively.

Published

2000

71. Pharmacokinetic study and determination of imperialine, the major bioactive component in antitussive Fritillaria cirrhosa, in rat by high-performance liquid chromatography coupled with evaporative light-scattering detector.

Author

Chan SW, Li SL, Lin G, and Li P

Subjects

Animals, Antitussive Agents analysis, Cevanes analysis, Light, Male, Rats, Rats, Sprague-Dawley, Scattering, Radiation, Antitussive Agents pharmacokinetics, Cevanes pharmacokinetics, Chromatography, High Pressure Liquid methods

Published

2000

72. Isolation and identification of three potential impurities of pholcodine bulk drug substance.

Author

Denk OM, Gray AI, Skellern GG, and Watson DG

Subjects

Antitussive Agents chemistry, Chloroform chemistry, Chromatography, High Pressure Liquid, Chromatography, Thin Layer, Codeine chemistry, Mass Spectrometry, Morpholines chemistry, Spectrophotometry, Ultraviolet, Antitussive Agents analysis, Codeine analogs & derivatives, Codeine analysis, Drug Contamination, Morpholines analysis

Abstract

Three previously unreported manufacturing impurities were isolated from a pholcodine mother liquor using preparative reversed-phase HPLC. The liquor was the residue remaining after recrystallisation of a production batch of pholcodine. The impurities, which are structurally related to pholcodine, were initially detected by thin-layer chromatography (TLC). Their structures were determined after separation by preparative HPLC (Econo-Prep 5 microm C18 column, 30 cm x 21.2 mm i.d.). Structure elucidation was carried out using nuclear magnetic resonance (NMR) spectroscopy, mass spectroscopy (MS) and ultra violet (UV) spectroscopy. The impurities were identified as alkylated derivatives of pholcodine possessing second 2-morpholinoethyl substituents at various positions.

Published

2000

73. Noscapine as an adulterant in illicit heroin samples.

Author

Klemenc S

Subjects

Gas Chromatography-Mass Spectrometry, Antitussive Agents analysis, Drug Contamination, Heroin chemistry, Illicit Drugs chemistry, Narcotics chemistry, Noscapine analysis

Abstract

In this short report the evidence is given (based on the analyses of 22 case samples) that noscapine can be used as an adulterant in illicit heroin samples. In this context, the appearance of illicit heroin samples characterised by a high noscapine content (up to 61%) and a high noscapine/whole morphine ratio (up to 3.5) is highlighted. All samples discussed in the paper (132) were seized in Slovenia, in the period from 1997 to 1999 and were analysed by gas chromatography-mass spectrometry.

Published

2000

74. Pre-column derivatization and gas chromatographic determination of alkaloids in bulbs of Fritillaria.

Author

Li SL, Chan SW, Li P, Lin G, Zhou GH, Ren YJ, and Chiu FC

Subjects

Cevanes analysis, Gas Chromatography-Mass Spectrometry, Alkaloids analysis, Antitussive Agents analysis, Chromatography, Gas methods, Drugs, Chinese Herbal chemistry

Abstract

A method of precolumn derivatization GC with FID detection was developed for a simultaneous analysis of five major steroidal alkaloids of Fritillaria species, namely ebeiedine, ebeiedinone, verticine, verticinone and imperialine. Derivatization was carried out by trimethylsilylation of the hydroxyl-containing Fritillaria alkaloids to the corresponding trimethylsilylates with trimethylsilylimidazole. Reaction conditions were optimised and the alkaloids derivatives were characterised by on-line GC-MS. The validated GC method demonstrated a good linearity at the sampling ranges used. This analytical method is simple, convenient and reproducible. The developed assay was successfully applied to the determination of the major pharmacologically active alkaloids in three commonly used antitussive Fritillaria species: F. cirrhosa, F. thunbergii and F. pallidiflora.

Published

1999

75. Characterization of cytochrome P-450 2D1 activity in rat brain: high-affinity kinetics for dextromethorphan.

Author

Tyndale RF, Li Y, Li NY, Messina E, Miksys S, and Sellers EM

Subjects

Alcohol Oxidoreductases, Animals, Antibodies, Blocking pharmacology, Antitussive Agents analysis, Cerebellum drug effects, Cerebellum metabolism, Chromatography, High Pressure Liquid, Cytochrome P-450 Enzyme Inhibitors, Cytochrome P450 Family 2, Dextromethorphan analysis, Dextrorphan analysis, Dextrorphan pharmacokinetics, Kinetics, Liver drug effects, Liver metabolism, Male, Membranes drug effects, Membranes metabolism, NADP metabolism, Neuroprotective Agents analysis, Neuroprotective Agents pharmacokinetics, Rats, Rats, Wistar, Antitussive Agents pharmacokinetics, Aryl Hydrocarbon Hydroxylases, Brain enzymology, Cytochrome P-450 Enzyme System metabolism, Dextromethorphan pharmacokinetics

Abstract

We investigated the enzymatic function, stability, and regional distribution of rat brain cytochrome P-450 (CYP) 2D1 activity. CYP2D1 is the homolog of human CYP2D6, a genetically variable enzyme that activates or inactivates many clinical drugs acting on the central nervous system (e.g., antidepressants, monoamine oxidase inhibitors, serotonin uptake inhibitors, and neuroleptics), drugs of abuse (e.g., amphetamine and codeine), neurotoxins (e.g., 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine, 1,2,3, 4-tetrahydroquinoline), and endogenous neurochemicals (e.g., tryptamine). The CYP2D family has been identified in rodent, canine, and primate brain. Conversion of dextromethorphan to dextrorphan by rat brain membranes was assayed by HPLC and was dependent on NADPH, protein concentration, and incubation time. Significant loss of activity was observed in some homogenizing buffers and after freezing of whole tissues or membrane preparations. Dextromethorphan (0.5-640 microM) metabolism was mediated by high- and low-affinity enzyme systems; K(m1) was 2.7 +/- 2.6 and K(m2) was 757 +/- 156 microM (n = 3 rats, mean +/- S.E.). The enzyme activity was significantly (p <.01) and stereoselectively inhibited by CYP2D1 inhibitors quinine and quinidine (not by CYP2C or CYP3A inhibitors), and by anti-CYP2D6 peptide antiserum (not by anti-CYP2C, -CYP2B, or -CYP3A antibodies). The enzymatic activity demonstrated significant brain regional variation (n = 10 regions, p <.001). These data characterize CYP2D1-mediated dextromethorphan metabolism in rat brain and suggest that localized metabolism of other CYP2D1 substrates (drugs, neurotoxins, and possibly endogenous compounds) within the brain will occur. In humans, CYP2D6 is genetically polymorphic; the variable expression of brain CYP2D6 may result in interindividual differences in central drug and neurotoxin metabolism, possibly contributing to interindividual differences in drug effects and neurotoxicity.

Published

1999

76. Fatal poisonings where ethylmorphine from antitussive medications contributed to death.

Author

Jonasson B, Jonasson U, Holmgren P, and Saldeen T

Subjects

Adult, Alcoholic Intoxication diagnosis, Alcoholic Intoxication pathology, Anti-Anxiety Agents analysis, Anti-Anxiety Agents poisoning, Antitussive Agents analysis, Autopsy legislation & jurisprudence, Benzodiazepines, Dose-Response Relationship, Drug, Ethylmorphine analysis, Female, Humans, Male, Middle Aged, Poisoning pathology, Substance-Related Disorders diagnosis, Substance-Related Disorders pathology, Sweden, Antitussive Agents poisoning, Cause of Death, Ethylmorphine poisoning, Poisoning etiology

Abstract

The hypothesis that antitussives containing ethylmorphine are abused by alcoholics and drug addicts and that this may lead to fatal poisonings where ethylmorphine causes or contributes to death was investigated. For this purpose 14 cases were analysed where a blood ethylmorphine concentration above the therapeutic level of >/= 0.3 microg/g was found in autopsy blood samples. Alcohol was found in 8 of the 14 cases and alcoholism or drug addiction was noted on 8 of the 14 death certificates. Other drugs, mostly benzodiazepines, were found in all 14 cases. The cause of death was fatal poisoning in 8 of the 14 cases and although there were no mono-intoxications, the cause of death was specified as fatal ethylmorphine poisoning in 2 cases. Among the unspecified medicinal drug poisonings there were five cases with very high blood levels of ethylmorphine, indicating that this drug played an important contribution to the cause of death. The results indicate that deaths due to ethylmorphine in antitussive medicines may occur among drug addicts and alcoholics taking it in overdose. Physicians should therefore be restrictive in prescribing cough mixtures containing ethylmorphine to these categories of patients. Prescription of large amounts of the drug should be avoided.

Published

1999

77. Determination of pseudoephedrine hydrochloride and carbinoxamine maleate in combination drug formulation by liquid chromatography.

Author

Mansour AM

Subjects

Dosage Forms, Drug Combinations, Linear Models, Reproducibility of Results, Antitussive Agents analysis, Chromatography, Liquid, Ephedrine analysis, Histamine H1 Antagonists analysis, Pyridines analysis

Abstract

An isocratic, reversed-phase liquid chromatographic (LC) method was developed for simultaneous determination of pseudoephedrine hydrochloride (I) and carbinoxamine maleate (II) in a pharmaceutical dosage form. Analysis was conducted on a CN column (10 microns), with a mobile phase consisting of acetonitrile-methanol-phosphate buffer (pH 5.3)-water (140 + 170 + 40 + 100) and at a detection wavelength of 262 nm. The method was validated for linearity, precision, system reproducibility, and accuracy. Recoveries at 80-120% of labeled claim ranged from 97.4 to 100.7% and from 98.5 to 100.2% for I and II, respectively. Results were linear (correlation coefficient, r > 0.9995 for I in the range 250-750 micrograms/mL and r > 0.9999 for II in the range 20-60 micrograms/mL.

Published

1998

78. Simultaneous determination of dextromethorphan HBr and bromhexine HCl in tablets by first-derivative spectrophotometry.

Author

Tantishaiyakul V, Poeaknapo C, Sribun P, and Sirisuppanon K

Subjects

Chromatography, High Pressure Liquid, Reproducibility of Results, Spectrophotometry, Ultraviolet methods, Antitussive Agents analysis, Bromhexine analysis, Dextromethorphan analysis, Expectorants analysis

Abstract

A rapid, simple and direct assay procedure based on first-derivative spectrophotometry, using a zero-crossing and peak-to-base measurement at 234 and 324 nm, respectively, has been developed for the specific determination of dextromethorphan HBr and bromhexine HCl in tablets. Calibration graphs were linear with the correlation coefficients of 0.9999 for both analytes. The limit of detections were 0.033 and 0.103 microgram ml-1 for dextromethorphan HBr and bromhexine HCl, respectively. A HPLC method has been developed as the reference method. The results obtained by the first-derivative spectrophotometry were in good agreement with those found by the HPLC method.

Published

1998

79. Capillary electrophoresis with electrospray mass spectrometry detection for low-molecular-mass compounds.

Author

Wheat TE, Lilley KA, and Banks JF

Subjects

Antitussive Agents chemistry, Buffers, Hydrogen-Ion Concentration, Molecular Weight, Peptides chemistry, Alkanesulfonates analysis, Antitussive Agents analysis, Coloring Agents analysis, Electrophoresis, Capillary methods, Mass Spectrometry methods, Peptides analysis

Abstract

Mass spectrometry (MS) detection using electrospray ionization (ESI) has been explored for the separation by capillary electrophoresis (CE) of a number of sample mixtures containing low-molecular-mass species. Optimal sheath liquid composition has been determined using a peptide mixture in which femtomolar quantities of analyte were easily observed. Effects of CE buffer choice were studied in detail. Also, a separation of basic drugs in cough syrup has been successfully detected by ESI-MS. Using negative ionization, a mixture of alkyl sulfonates and a mixture of food dyes were analyzed. All components were easily resolved and identified by molecular weight.

Published

1997

80. Simultaneous determination of bromhexine hydrochloride and methyl and propyl p-hydroxybenzoate and determination of dextromethorphan hydrobromide in cough-cold syrup by high-performance liquid chromatography.

Author

Rauha JP, Salomies H, and Aalto M

Subjects

Chromatography, High Pressure Liquid methods, Antitussive Agents analysis, Bromhexine analysis, Dextromethorphan analysis, Expectorants analysis, Parabens analysis

Abstract

Liquid chromatographic methods were developed for the determination of bromhexine hydrochloride, methyl p-hydroxybenzoate and propyl p-hydroxybenzoate (method A) and dextromethorphan hydrobromide (method B) in cough-cold syrup formulations. Reversed-phase analytical columns (150 mm x 3.9 mm i.d.) were used with (A) C18 and (B) phenyl as stationary phases and mixtures of (A) acetonitrile and aqueous 15 mM triethylamine solution (43:57) and (B) methanol and aqueous 3% ammonium formate buffer solution (53:47) as mobile phases at a flow rate of 1.0 ml min-1. Both aqueous components were adjusted to pH 3.9. UV detection of analytes was at (A) 245 nm and (B) 278 nm. In both methods, the time required for an HPLC run giving good separations and recoveries was less than 8 min.

Published

1996

81. Determination of noscapine, hexylresorcinol and anethole in cough lozenges by liquid chromatography.

Author

Lucangioli S, Fernández Otero G, Rodríguez V, and Carducci CN

Subjects

Chromatography, Liquid, Indicators and Reagents, Tablets, Anethole Trithione analysis, Antitussive Agents analysis, Hexylresorcinol analysis, Noscapine analysis

Abstract

A liquid chromatographic method was developed for the simultaneous separation and determination of noscapine hydrochloride, hexylresorcinol and anethole in cough lozenges. Analysis was performed on a phenyl column with phosphate buffer- acetonitrile as mobile phase and the separated components were detected at 282 mm. Recoveries obtained for the analytes were of 94.6% for noscapine hydrochloride, 99.1% for hexylresorcinol and 96.3% for anethole. The values of the relative standard deviation were 0.8% for noscapine hydrochloride, 1.5% for hexylresorcinol and 1.1% for anethole. The analytical method was validated and a system suitability test was accomplished for the chromatographic method.

Published

1996

82. Large-volume sample stacking of selected drugs of forensic significance by capillary electrophoresis.

Author

McGrath G and Smyth WF

Subjects

Anti-Anxiety Agents analysis, Anti-Anxiety Agents chemistry, Antitussive Agents analysis, Antitussive Agents chemistry, Bronchodilator Agents analysis, Bronchodilator Agents chemistry, Cetrimonium, Cetrimonium Compounds chemistry, Clenbuterol analysis, Clenbuterol chemistry, Codeine analysis, Codeine chemistry, Detergents chemistry, Flurazepam analysis, Flurazepam chemistry, Hydrogen-Ion Concentration, Meperidine analysis, Meperidine chemistry, Narcotics analysis, Narcotics chemistry, Noscapine analysis, Noscapine chemistry, Reproducibility of Results, Spectrophotometry, Ultraviolet, Surface Properties, Time Factors, Chemistry, Clinical methods, Electrophoresis, Capillary methods, Forensic Medicine methods, Pharmaceutical Preparations analysis, Pharmaceutical Preparations chemistry

Abstract

Large-volume sample stacking capillary electrophoresis (LVSS-CE) and conventional capillary electrophoresis (CE) are compared for the separation of drugs of significance to forensic and clinical analyses. LVSS-CE for cations requires the use of an electroosmotic flow (EOF) modifier in conjunction with polarity switching to effect on-column concentration of an analyte and its subsequent migration in the capillary. The run buffer consists of 0.05 mol dm(-3) disodium tetraborate adjusted to pH 2.2 with orthophosphoric acid, and the EOF modifier is 0.002 mol dm(-3) cetyltrimethylammonium bromide. CE investigations used an identical run buffer minus the EOF modifier. LVSS-CE and CE investigations used injection times of 30 s and 3 s, respectively. Both modes of capillary electrophoresis are compared in terms of their limits of detection, efficiency, resolution and reproducibility. LVSS-CE is also applied to the analysis of a spiked urine sample.

Published

1996

83. Fatal zipeprol and dextromethorphan poisonings in Korea.

Author

Yoo Y, Chung H, Kim E, and Kim M

Subjects

Adult, Antitussive Agents analysis, Antitussive Agents blood, Calibration, Chromatography, Gas, Dextromethorphan analysis, Dextromethorphan blood, Dose-Response Relationship, Drug, Female, Gastrointestinal Contents chemistry, Humans, Illicit Drugs analysis, Illicit Drugs blood, Korea epidemiology, Male, Piperazines analysis, Piperazines blood, Poisoning epidemiology, Poisoning mortality, Antitussive Agents poisoning, Dextromethorphan poisoning, Illicit Drugs poisoning, Piperazines poisoning

Abstract

Zipeprol and dextromethorphan are abused together by young people in Korea to obtain a stronger hallucinogenic effect. Because large amounts of these drugs are taken for this reason, nine fatal poisonings due to zipeprol and dextromethorphan have been reported since 1993. In this paper, the concentration of drugs in the postmortem blood and gastric contents of these victims is examined. The determination and identification of the drugs in biological fluids were conducted by gas chromatography (GC)-thermionic specific detection and GC-mass spectrometry. Linear calibration curves and high recoveries were obtained. The blood concentrations of zipeprol varied from 1.3 to 28.6 micrograms/mL, and the concentrations of dextromethorphan ranged from 1.1 to 18.3 micrograms/mL. The concentration of zipeprol in the gastric contents ranged from 26.8 to 1384.8 micrograms/g, and dextromethorphan concentrations varied from 2.1 to 243.7 micrograms/g.

Published

1996

84. Detection of codeine and phenobarbital in sweat collected with a sweat patch.

Author

Kintz P, Tracqui A, Jamey C, and Mangin P

Subjects

Administration, Oral, Adult, Antitussive Agents administration & dosage, Antitussive Agents analysis, Arm, Back, Codeine administration & dosage, Codeine analysis, Female, Gas Chromatography-Mass Spectrometry, Humans, Hypnotics and Sedatives administration & dosage, Hypnotics and Sedatives analysis, Male, Medical Laboratory Personnel, Morphine administration & dosage, Morphine metabolism, Morphine urine, Phenobarbital administration & dosage, Phenobarbital analysis, Reference Standards, Ribs, Specimen Handling, Antitussive Agents pharmacokinetics, Codeine pharmacokinetics, Hypnotics and Sedatives pharmacokinetics, Phenobarbital pharmacokinetics, Sweat metabolism

Abstract

Six male and two female subjects participated in a clinical study to determine the time course, the cumulative excretion, the intrasubject variability, the influence of site application, and the concentrations of codeine or phenobarbital in sweat following administration of a single dose of the drug. The doses of codeine and phenobarbital were 90 and 100 mg. respectively. Sweat was collected by means of a Sudormed sweat patch. Patches were removed at specified times over 1 week, and the drug content was determined by gas chromatography-mass spectrometry using deuterated internal standards. Codeine was detectable at 1 h following the administration, and a plateau concentration was observed on the third day. The peak codeine concentration was observed during the 12-24-h period. Morphine was never detected in sweat. In contrast, phenobarbital was first observed 3 h after administration, and cumulative excretion was continual throughout the week. Intersubject variability was enormous, as the concentrations for the same dose were in a magnitude of 1-5. Concentrations were in the range of 2-127 and 0.5-33 ng per patch for codeine and phenobarbital, respectively. The influence of the site of patch application was evaluated by analysis of six patches, all removed at the same time (24 h) in two subjects receiving 90 mg codeine. Codeine concentrations differed by a magnitude of 1-3 according to the area of application: the upper arm, the back, and the ribs. These data suggest that the sweat patch technology can be useful for documenting drug use over a 1-week period of surveillance.

Published

1996

85. [Experimental studies on the quality control of xiaoluo pills].

Author

Zhen H and Yang Y

Subjects

Calcium Carbonate analysis, Chromatography, Thin Layer, Densitometry, Drug Combinations, Quality Control, Antitussive Agents analysis, Cevanes analysis, Drugs, Chinese Herbal chemistry

Abstract

Microscopic and physico-chemical methods have been used in the qualitative study of Xiaoluo Pills. The contents of peimine, peiminine and calcium carbonate in these pills have been determined. The proposed method can be used to control the quality of Xiaoluo Pills.

Published

1996

86. [Determination of genkwanin in flos Genkwa by HPLC].

Author

Zhang B, Yuan S, and Xia K

Subjects

Chromatography, High Pressure Liquid, Antitussive Agents analysis, Drugs, Chinese Herbal chemistry, Flavones, Flavonoids analysis

Abstract

In this paper, the method for determining genkwanin in Flos Genkwa was established by HPLC. Detected at 332nm on a Lichrosorb 5 RP-18 column with a mobile phase of methanol-water-acetic acid (65:35:5), the content of genkwanin in Flos Genkwa was determined to be 0.16%. The recovery rate was 95.46% and RSD 1.15%.

Published

1996

87. Determination of guaiphenesin in anti-tussive pharmaceutical preparations containing dextromethorphan by first- and second-derivative ultraviolet spectrophotometry.

Author

Lee AR and Hu TM

Subjects

Reproducibility of Results, Solutions analysis, Tablets analysis, Antitussive Agents analysis, Dextromethorphan analysis, Guaifenesin analysis, Spectrophotometry, Ultraviolet methods

Abstract

Rapid, simple and direct assay procedures based on selective first (D1)- and second (D2)-derivative spectrophotometry, using a zero-crossing technique of measurement at 279.2 and 280.0 nm, respectively, have been developed for the specific determination of guaiphenesin in the presence of dextromethorphan, drugs with closely overlapping absorption spectra, in synthetic admixtures and in pharmaceutical dosage forms (tablets and syrups). The methods do not require extraction with organic solvents and are easier to perform than their conventional counterparts. Calibration graphs were linear (r = 0.99999 for D1 and 0.99969 for D2, respectively). Good selectivity, accuracy and precision were found. However, the performance of the analysis of guaiphenesin by the second-derivative mode deteriorated when the ratio of dextromethorphan to guaiphenesin was greater than one. Thus, the first-derivative spectrophotometry is the method of choice for the assay of tablets and syrups containing the two drugs.

Published

1994

88. GC-MS procedure for the analysis of zipeprol.

Author

Kintz P, Flesch F, Jaeger A, and Mangin P

Subjects

Adult, Antitussive Agents blood, Antitussive Agents poisoning, Gas Chromatography-Mass Spectrometry, Gastrointestinal Contents chemistry, Humans, Indicators and Reagents, Levallorphan analysis, Male, Piperazines blood, Piperazines poisoning, Solvents, Suicide, Attempted, Antitussive Agents analysis, Piperazines analysis

Abstract

A sensitive and specific quantitative method for the determination of zipeprol, a newly abused antitussive, in human fluids is described. Zipeprol and an internal standard, levallorphan, are isolated by a basic extraction and back-extraction process. The final extract is derivatizated with BSTFA + 1% TMCS and separated on a 12-m HP-1 capillary column. Drugs are detected by selected ion monitoring at m/z 335 and m/z 355 for zipeprol and the internal standard, respectively. The minimum detectable quantities are 0.6 and 0.4 ng ml-1, for zipeprol in plasma and urine, respectively. Relative standard deviations for within-run data are less than 6%.

Published

1993

89. [Antitussive action of extracts and polysaccharides of marsh mallow (Althea officinalis L., var. robusta)].

Author

Nosál'ova G, Strapková A, Kardosová A, Capek P, Zathurecký L, and Bukovská E

Subjects

Animals, Antitussive Agents pharmacology, Cats, Cough physiopathology, Female, Male, Physical Stimulation, Plant Extracts pharmacology, Polysaccharides analysis, Polysaccharides pharmacology, Antitussive Agents analysis, Plants, Medicinal chemistry

Abstract

The complex extract and the polysaccharide isolated from the roots of marsh mallow were tested for antitussive activity in unanaesthetized cats of both sexes. Cough was elicited by mechanical stimulation of laryngopharyngeal and tracheobronchial mucous area of the respiratory system with a Nylon fibre (diameter 0.35 mm). Cough was evaluated on the basis of the changes in lateral tracheal pressure. The polysaccharide and the complex extract were administered p.o. in a dose of 50 and 100 mg/kg b.w., respectively. The efficiency of the mentioned compounds was compared with the cough-suppressing effect of drugs belonging to the non-narcotic antitussics. The results of the experiments showed that administration of the polysaccharide led to a statistically significant decrease of the number of cough efforts both from laryngopharyngeal and tracheobronchial areas of the the respiratory system. The polysaccharide in a dose of 50 mg/kg b.w. was as effective in inhibition of the cough reflex as Sirupus Althaeae in a dose of 1000 mg/kg b.w. and more effective than prenoxdiazine in a dose of 30 mg/kg b.w. However, the cough-suppressing effect of the polysaccharide was lower than that of dropropizine. The extract was less effective than the polysaccharide.

Published

1992

90. Dextromethorphan poisoning reversed by naloxone.

Author

Schneider SM, Michelson EA, Boucek CD, and Ilkhanipour K

Subjects

Adolescent, Adult, Antitussive Agents analysis, Antitussive Agents poisoning, Child, Preschool, Dextromethorphan analysis, Drug Overdose, Female, Humans, Infant, Male, Poisoning complications, Poisoning drug therapy, Antidotes therapeutic use, Dextromethorphan poisoning, Naloxone therapeutic use

Abstract

Dextromethorphan, a common ingredient in cough syrups, has rarely been described to cause toxicity. The authors describe an unusual case of a known asthmatic presenting with somnolence, who appeared to be in end-stage respiratory failure. Her partial response to routine naloxone, 1 mg, was surprising. However, additional naloxone was required to completely normalize the patient's mental status. The authors suggest naloxone be administered in doses of 0.4 mg or more intravenously in suspected dextromethorphan overdose.

Published

1991

91. Determination of chlorpheniramine maleate, dihydrocodeine bitartrate and ephedrine hydrochloride in cough mixture by derivative and differential spectrometry.

Author

Korany MA, Bedair MM, and el-Gindy A

Subjects

Codeine analysis, Drug Combinations, Indicators and Reagents, Spectrophotometry, Ultraviolet, Antitussive Agents analysis, Chlorpheniramine analysis, Codeine analogs & derivatives, Ephedrine analysis

Abstract

A method is presented for the determination of chlorpheniramine maleate, dihydrocodeine bitartrate and ephedrine hydrochloride in a three-component mixture without prior separation. Chlorpheniramine maleate was determined by the first and second derivative-differential spectrophotometry, while dihydrocodeine bitartrate was directly determined using first and second derivative measurements. Ephedrine hydrochloride could be determined by first and second derivative spectrophotometry after its oxidation with sodium metaperiodate. The method was proved using synthetic mixtures of these drugs and was applied for their determination in syrup with a coefficient of variation less than 2%.

Published

1990

92. Determination of enantiomeric purity of ephedrine and pseudoephedrine by high-performance liquid chromatography with dual optical rotation/UV absorbance detection.

Author

Wu ZC, Goodall DM, and Lloyd DK

Subjects

Antitussive Agents analysis, Chromatography, High Pressure Liquid methods, Ephedrine analysis, Mathematics, Optical Rotation, Spectrophotometry, Ultraviolet methods, Stereoisomerism, Ephedrine chemistry

Abstract

A reversed-phase high-performance liquid chromatography (HPLC) method with dual optical rotation/UV absorbance detection has been developed for the determination of enantiomeric purity of ephedrine hydrochloride and pseudoephedrine hydrochloride using an achiral column. The method gave a correlation coefficient of 0.9997 for the plot of log(optical rotation response) versus log (concentration) over the range of 0.06-10 mg ml(-1) of (+)-ephedrine hydrochloride (20 microliters injection). The limit of detection was 1.0 micrograms. Enantiomeric purity is shown to be most readily determined by measuring optical rotation, alpha, and absorbance, A, responses for standard and unknown samples, and using the equation (alpha/A)u/(alpha/A)s = (2xu - 1)/(2xs - 1), where x is the mole fraction of one of the enantiomers and subscripts s and u refer to standard and unknown, respectively. In blind trials using unknown mixtures of (+)- and (+/-)-ephedrine hydrochloride and a (+)-ephedrine hydrochloride standard, enantiomeric purities were determined to +/- 0.4% (95% confidence level) with five or six replicate 50 micrograms injections. The method has also been applied to the determination of the enantiomer mole fraction of (+)-pseudoephedrine hydrochloride in a cough linctus, giving xu = 0.99 +/- 0.01 with seven replicate injections of 20-fold diluted linctus samples containing 7.5 micrograms of the chiral compound being assayed. Unlike conventional polarimetry, the method does not require chemically-pure samples and can be orders of magnitude more economical in material.

Published

1990

93. The application of quadrupole mass filters in field desorption mass spectrometry.

Author

Gierlich HH, Heinen HJ, and Beckey HD

Subjects

Adsorption, Antitussive Agents analysis, Benzhydryl Compounds analysis, Filtration, Humans, Hypnotics and Sedatives analysis, Mass Spectrometry instrumentation, Meclizine analysis, Pemoline analysis, Propanolamines analysis, Hypnotics and Sedatives urine, Mass Spectrometry methods

Abstract

The advantages and limitations which quadrupole mass filters afford to the field desorption technique with respect to use for routine work are discussed and experimentally confirmed by the analyses of some drugs using a field desorption quadrupole mass spectrometer. The possibility of fast identification of drug intoxication is demonstrated by the analysis of the chloroform extract of urine in a case of overdose of hypnotics.

Published

1975

94. The physician's role in reducing patient exposure to sucrose.

Author

Shannon IL and Edmonds EJ

Subjects

Antitussive Agents analysis, Child Nutritional Physiological Phenomena, Dental Caries etiology, Humans, Vitamins analysis, Dietary Carbohydrates adverse effects, Dietary Carbohydrates analysis, Sucrose adverse effects, Sucrose analysis

Published

1977

95. Colorimetric determination of pentoxiverine citrate in some pharmaceutical preparations.

Author

Weclawska K and Regosz A

Subjects

Colorimetry, Antitussive Agents analysis, Cyclopentanes analysis

Published

1987

96. [The identification and total synthesis of aichasu, an antitussive agent (author's transl)].

Author

Xie JX, Wang L, Liu CX, and Zhang DY

Subjects

Animals, Antitussive Agents analysis, Benzopyrans isolation & purification, China, Humans, Mice, Middle Aged, Plant Extracts analysis, Antitussive Agents chemical synthesis, Benzopyrans chemical synthesis, Plants, Medicinal

Published

1981

97. Simultaneous determination of acetaminophen, guaifenesin, pseudoephedrine, pholcodine, and paraben preservatives in cough mixture by high-performance liquid chromatography.

Author

Carnevale L

Subjects

Acetaminophen analysis, Chromatography, High Pressure Liquid methods, Codeine analogs & derivatives, Codeine analysis, Drug Combinations, Ephedrine analysis, Guaifenesin analysis, Morpholines analysis, Parabens analysis, Antitussive Agents analysis

Abstract

The separation and simultaneous determination, by high-performance liquid chromatography, of acetaminophen (I), guaifenesin (II), pseudoephedrine hydrochloride (III), and pholcodine (IV), together with a series of parabens (methyl to butyl, V-VIII) in a cough mixture, has been demonstrated using a chemically bonded octadecylsilane stationary phase with a mobile phase of methanol-water-acetic acid (45:55:2) containing the ion-pairing agent octanesulfonic acid. Retention volumes for the active ingredients were 3.8 ml, 5.4 ml, 9.4 ml, and 15.6 ml for compounds I-IV, respectively. Corrected retention volumes for the parabens [5.4 ml for methyl (V), 9.6 ml for ethyl (VI), 18.5 ml for propyl (VII), and 37.9 ml for butyl (VIII)] showed an exponential relationship with chain length of the esterifying alcohols. Excipients did not interfere with the estimation of any of the compounds, hence pretreatment of the sample was unnecessary. Average recoveries of the active ingredients and of the parabens from laboratory prepared samples were essentially 100% of theoretical with standard deviations of 1.7, 0.3, 1.5, 0.3, 0.3, 3.3, 0.7, and 2.7% for I-VIII, respectively.

Published

1983

98. Determination of phenylpropanolamine hydrochloride as benzaldehyde in pharmaceutical preparations using normal-phase high-performance liquid chromatography.

Author

Taylor P, Braddock PD, and Ross S

Subjects

Antitussive Agents analysis, Benzaldehydes analysis, Chromatography, High Pressure Liquid methods, Dosage Forms analysis, Phenylpropanolamine analysis

Published

1984

99. Analysis of cough/cold products using an adamantyl column.

Author

Yang SS and Gilpin RK

Subjects

Adamantane, Chromatography, High Pressure Liquid, Solutions, Tablets, Antitussive Agents analysis

Abstract

High-performance liquid chromatographic methods are developed for the determination of active ingredients in several cough/cold preparations. A novel adamantyl phase is used in combination with either totally aqueous or high aqueous hydroorganic mobile phases.

Published

1988

100. Colorimetric determinations of chlorpheniramine maleate, ephedrine hydrochloride, and guaiacolsulfonate potassium in a cough syrup.

Author

Das Gupta V and de Lara AJ

Subjects

Colorimetry, Methods, Antitussive Agents analysis, Chlorpheniramine analysis, Ephedrine analysis, Guaiacol analysis

Abstract

Colorimetric methods for the quantitative determinations of chlorpheniramine maleate, ephedrine hydrochloride, and guaiacolsulfonate potassium in a cough syrup containing color (amaranth) are reported. Chlorpheniramine maleate can be assayed using the cyanogen bromide method as reported in the literature. Ephedrine hydrochloride can be assayed using a dye method in which interference from chlorpheniramine maleate is taken into consideration. Guaiacolsulfonate potassium can be assayed by coupling it with 4-aminoantipyrine (the method is similar to the one for phenylephrine hydrochloride). All of the methods are simple, accurate, and precise. The application of the guaiacolsulfonate potassium assay method to commercial dosage forms is reported.

Published

1975