Chromatography of Suspensions – An Experimental and Theoretical Investigation of Axial Dispersion Phenomena

Abstract

Herein is reported an experimental and theoretical investigation of axial dispersion phenomena in the chromatography of spherical suspensions in the submicron range. Peak separation and broadening were measured for a number of particle suspensions (polystyrene, polyvinylacetate, styrene-acrylic acid copolymer, butadiene-acrylonitrile copolymer latices and silica particles) using different column combinations containing porous inorganic packing materials (Fractosils, Bioglass, Corning Glass) and over a wide range of carrier fluid (water containing 1 g/l Aerosol O.T. and 1 g/l potassium nitrate) flowrates. Peak separation was virtually independent of carrier fluid flowrate while peak broadening increased significantly. Analytical solutions of the integral equation which describes axial dispersion in the chromatography of suspensions have been found for a general detector which includes light scattering, refractometer and viscosity-concentration detectors. These solutions were used to obtain dispersion corrections for various particle diameter averages (number, surface, weight and volume). Corrections to number and surface average particle diameters for axial dispersion are excessive with a light scattering detector. These large corrections are related to the fact that in the Rayleigh scattering regime, the extinction coefficient is proportional to diameter to the fourth power. The refractometer gives reasonable dispersion corrections for all particle diameter averages. The theoretical equations derived herein are equally applicable to hydrodynamic chromatography (HDC) and capillary particle chromatography (CPC).     

An Automated Method for the Determination of Enoximone and Its Major Sulfoxide Metabolite in Plasma Using Robotic Technology–High Performance Liquid Chromatography

Abstract

An automated analytical procedure for the determination of enoximone, a new cardiotonic agent, and its major oxidative metabolite in plasma using robotic technology is described. A Zymark robot is used to perform all the operations of solid phase extraction including column pretreatment, internal standard addition, sample mixing, sample pipetting, column rinsing, drying and sample elution. The processed sample is injected directly into the high performance liquid chromatography system which is equipped with an ultraviolet absorption detector. The assay has good precision and accuracy, equivalent to the manual method it replaces, and yet provides higher throughput of sample.     

Liquid Chromatography‐Electrospray Ionization Mass Spectrometric Method for Determination of Gliclazide in Human Plasma

Abstract

A rapid, sensitive, and specific liquid chromatography‐electrospray ionization mass spectrometric (LC‐ESI‐MS) method has been developed for quantification of gliclazide in human plasma. The analyte and tolbutamide (internal standard, I.S.) were extracted from plasma samples with n‐hexane–dichloromethane (1:1, v/v) and analyzed on a C₁₈ column. The chromatographic separation was achieved within 4.0 min by using methanol–0.5% formic acid (80:20, v/v) as mobile phase and the flow rate was 1.0 mL/min. Ion signals m/z 324.0 and 271.0 for gliclazide and internal standard were measured in the positive mode, respectively. The method was linear within the range of 2.5–2000 ng/mL. The lower limit of quantification (LLOQ) was 2.5 ng/mL. The intra‐ and inter‐day precisions were lower than 2.8% in terms of relative standard deviation (RSD). The inter‐day relative error (RE) as determined from quality control samples (QCs) ranged from ?1.93% to 1.85%. This validated method was successfully applied for the evaluation of pharmacokinetic profiles of gliclazide modified‐release tablets in 20 healthy volunteers.     

Retention Time Locking in the Determination of Narcotic Drugs by Chromatography and Chromatography–Mass Spectrometry

The use of retention time locking (RTL) in the development of unified procedures for the detection and quantitative determination of drugs in biological fluids was considered. With consideration for the use of RTL, a chromatographic procedure with flame-ionization and mass-selective detection was developed for the detection and quantitative determination of opiates and their synthetic analogs; phenylalkylamine derivatives; cocaine; ketamine; and other narcotic drugs, their derivatives, and metabolites in urine. The analytical ranges for chromatography–mass spectrometry were 0.05–1000 and 0.005–1000 g/mL under the conditions of total ion current (TIC) scanning and selected ion monitoring (SIM), respectively. With flame-ionization detection (GC–FID), the analytical range was 0.5–1000 g/mL.     

Prospects for Using Chromatography–Mass Spectrometry for the Determination of Lipids in Clinical Cardiolipidology

Journal of Analytical Chemistry - Cardiolipidology – a new direction in cardiology – is developing intensively owing to the method of mass spectrometry. This method has acquired...     

An Efficient and Convenient Cyclization Method for the Synthesis of Flavans

Flavansrefertoalargegroupofnaturallyoccurringcompoundspossessinga2-phenyl-chromannucleus.Naturallyoccurringflavansexhibitanumberofimportantbiologicalactivitieswhichifexploitedproperly,mayleadtovaluablenewdrugsoragrochemicals'.Inflavansynthesis,thekeystepistoconstructthe3,4-dihydrobenzopyranring-Variousmethodshavebeendevelopedfortheringformation,butmostoftheminvolvemultiplestepsandgivelowoverallyields2.Inthispaper,BF3wasusedforthefirsttimeasanefficientcatalysttoformthepyranringfroml,3-diaryIp…     

Stability-Indicating Liquid Chromatography–Spectrophotometric UV Method for the Simultaneous Determination of Marbofloxacin,Dexamethasone and Clotrimazole in a Liquid Pharmaceutical Dosage Form

A novel, simple and reliable reversed-phase liquid chromatography (LC)–spectrophotometric UV stability-indicating method was developed and validated for the simultaneous assay of marbofloxacin, clotrimazole and dexamethasone acetate in the presence of their impurities and degradation products in a pharmaceutical formulation for veterinary use. A C18 (75 × 4.6 mm, 4 µm) column was used with an acetonitrile–ammonium acetate mixture as mobile phase delivered with gradient elution. A diode-array detection was used in the 200–400 nm range and the detection wavelength was set at 260 nm. Validation carried out on the pharmaceutical dosage form, according to Veterinary International Conference on Harmonization guidelines, demonstrated excellent specificity, linearity, precision, accuracy and robustness. Excellent specificity with respect to vehicle and degradation products obtained after forced degradation (i.e., oxidation, acid, alkaline and thermal degradation) was demonstrated. As for linearity, the LC–UV assay method is applicable in the 0.180–0.420 mg mL^?1 concentration range for marbofloxacin (r ² = 0.99), 0.060–0.140 mg mL^?1 for dexamethasone acetate (r ² = 0.97) and 0.600–1.400 mg mL^?1 for clotrimazole (r ² = 0.98). Very good repeatability (RSD < 0.8 %) and inter-day precision (RSD < 2.5 %) were observed for all analytes. Accuracy was in the 93–104 %, 98–111 % and 99–108 % confidence interval (95 %) for marbofloxacin, dexamethasone acetate and clotrimazole, respectively. The variations (±20 %) of mobile phase flow rate and pH, and oven column temperature did not exhibit an impact on the analyte content accuracy, demonstrating the robustness of the method. The LC–UV method here developed and validated may be used routinely for quality control.     

Stability-Indicating Liquid Chromatography–Spectrophotometric UV Method for the Simultaneous Determination of Marbofloxacin,Dexamethasone and Clotrimazole in a Liquid Pharmaceutical Dosage Form

A novel, simple and reliable reversed-phase liquid chromatography (LC)–spectrophotometric UV stability-indicating method was developed and validated for the simultaneous assay of marbofloxacin, clotrimazole and dexamethasone acetate in the presence of their impurities and degradation products in a pharmaceutical formulation for veterinary use. A C18 (75 × 4.6 mm, 4 µm) column was used with an acetonitrile–ammonium acetate mixture as mobile phase delivered with gradient elution. A diode-array detection was used in the 200–400 nm range and the detection wavelength was set at 260 nm. Validation carried out on the pharmaceutical dosage form, according to Veterinary International Conference on Harmonization guidelines, demonstrated excellent specificity, linearity, precision, accuracy and robustness. Excellent specificity with respect to vehicle and degradation products obtained after forced degradation (i.e., oxidation, acid, alkaline and thermal degradation) was demonstrated. As for linearity, the LC–UV assay method is applicable in the 0.180–0.420 mg mL⁻¹ concentration range for marbofloxacin (r ² = 0.99), 0.060–0.140 mg mL⁻¹ for dexamethasone acetate (r ² = 0.97) and 0.600–1.400 mg mL⁻¹ for clotrimazole (r ² = 0.98). Very good repeatability (RSD < 0.8 %) and inter-day precision (RSD < 2.5 %) were observed for all analytes. Accuracy was in the 93–104 %, 98–111 % and 99–108 % confidence interval (95 %) for marbofloxacin, dexamethasone acetate and clotrimazole, respectively. The variations (±20 %) of mobile phase flow rate and pH, and oven column temperature did not exhibit an impact on the analyte content accuracy, demonstrating the robustness of the method. The LC–UV method here developed and validated may be used routinely for quality control.

     

RP‐HPLC Method for the Determination of Tenofovir in Pharmaceutical Formulations and Spiked Human Plasma

Abstract

A simple reverse‐phase high‐performance liquid chromatographic method for the determination of tenofovir disoproxil fumarate (TDF) in pharmaceutical formulations and human plasma samples has been developed and validated. Piroxicam (PRX) was used as an internal standard. The assay of the drug was performed on a CLC C₁₈ (5 μ, 25 cm×4.6 mm i.d.) with UV detection at 259 nm. The mobile phase consisted of acetonitrile–water mixture in the ratio of 75∶25, and a flow rate of 1 ml/min was maintained. The standard curve was linear over the range of 0.2–10 µg/ml (r ²=0.9966). Analytic parameters have been evaluated. Within‐day and between‐day precision as expressed by relative standard deviation was found to be less than 2%. The method has been applied successfully for the determination of TDF in spiked human plasma samples and pharmaceutical formulations.     

An Ionic Liquid Loaded β-Cyclodextrin-Cross-Linked Polymer as the Solid Phase Extraction Material Coupled with High-Performance Liquid Chromatography for the Determination of Rhodamine B in Food

A novel method for separation and determination of rhodamine B in food samples is described. The work is based on the utilization of an ionic liquid loaded β-cyclodextrin cross-linked polymer coupled with high-performance liquid chromatography for the determination of rhodamine B. The inclusion interaction of the ionic liquid-β-cyclodextrin cross-linked polymer with rhodamine B was studied by FTIR. Under optimum conditions, the preconcentration factor achieved for this method was approximately 20. The linear range, detection limit, and relative standard deviation were 0.80 to 130.0 µg L^?1, 0.09 µg L^?1, and 0.66% (n = 3, concentration = 10.0 µg L^?1), respectively. The technique was successfully applied for determination of rhodamine B in food samples.     

Development and Validation of a Reverse-phase High Performance Liquid Chromatography Method for Determination of Exenatide in Poly（lactic-co-glycolic acid） Microspheres

Exenatide(synthetic exendin-4), which has been approved by the Food and Drug Administration(FDA) for the adjunctive treatment of patients with type 2 diabetes, is an incretin mimetic agent. The development and validation of a RP-HPLC method for the quantification of the exenatide in poly(lactic-co-glycolic acid)(PLGA) microspheres is described. Separation was performed on a C4 column via a mobile phase consisting of ACN:KH2PO4(0.02 mol/L, pH=2.5) gradient elution from 30:70 to 45:55(volume ratio) in 30 min. Multi-diode array detection(DAD) appears to be most appropriate to evaluate the spectral purity of exenatide. The limits of detection and quantification of exenatide were 0.4 and 1.2 μg/mL, respectively. The calibration curve of exenatide was linear in a range of 0.025―0.2 mg/mL with a correlation coefficient of 0.9995. The results of validation study show that this method is specific, accurate(recovery95%), precise(RSD2.0%) and robust.     

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.

     

An Improved Method for the Synthesis of Optically Active Tomoxetines and Fluoxetines

A chemoenzymatic approach was applied to the preparation of chiral 3-hydroxy-3-arylpropionates and 3-hydroxy-4,4,4-trifluombutanoate that are potential precursors for certain chiral pharmaceuticals including chiral tomoxetines and fluoxetines.     

Development and Validation of a GC–MS Method for the Determination of Methyl and Ethyl Camphorsulfonates in Esomeprazole Magnesium

A rapid gas chromatography–mass spectrometry method for the identification and determination of two carcinogenic impurities viz. methyl camphorsulfonate (MCS) and ethyl camphorsulfonate (ECS) in esomeprazole magnesium (EOM) is developed for the first time. The factors affecting method development and the fragmentation patterns of MCS and ECS based on the mass spectral analysis are described. The limit of detection and limit of quantitation values for both compounds were established as 3 and 10 ppm, respectively with respect to 50 mg mL^?1 of EOM. The method is linear within the range of 10–120 ppm and found to be precise, accurate, specific and robust.     

Development and Validation of a HPLC Method for the Determination of Five Bioactive Compounds in the “Xuebijing” Injection

A reversed phase high performance liquid chromatographic (RP-HPLC) method with ultraviolet (UV) detector was developed for simultaneously determining five bioactive components (i.e., hydroxysafflor yellow A: HSYA; paeoniflorin, ferulic acid, benzoic acid, and danshensu) in “Xuebijing” (XBJ) injection, a widely used traditional Chinese medicine (TCM) for treating sepsis and multiple organ dysfunction syndrome. A Zorbox SB C₁₈ column was used with 0.2% phosphoric acid (V/V)-acetonitrile as the mobile phase under the condition of gradient elution. The five components were analyzed by using a timed wavelength measure according to their maximum absorption wavelength. The intraday and interday precisions of the five investigated compounds were less than 1.17% and the average recoveries ranged from 97.3% to 103.2%. There were good linear correlations between the concentrations of the five components and their chromatographic peak areas (R² ≥ 0.9998), the proposed method was successfully applied to determine the five components in different batches of XBJ injection products, the results indicated that the proposed method is simple, stable, and accurate and could be readily utilized as a quality control method for manufacturing process of XBJ injection.     

Novel Sampling for the Determination of Naphthalene in Air by Gas Chromatography–Mass Spectrometry

Here are reported two new sampling method approaches for the determination of naphthalene in ambient air for concentrations from 0.25 to 18.7?µg/L. The first method used for gas phase naphthalene analysis produced an average recovery of 88.8% and the second method using headspace sampling produced an average recovery of 93.8%. The second method showed better recovery than the former, so it was used for subsequent comparative gas-phase determination of naphthalene. The second method was validated at various naphthalene concentrations and humidity using a naphthalene gas generator to produce various naphthalene standards and a naphthalene-monitoring instrument. The naphthalene concentrations generated using the gas generator and determined second sampling method with gas chromatography–mass spectrometry (GC–MS) were compared to the sensor measurements and were in good agreement. In summary, the sampling methods presented provided reliable gas-phase naphthalene determination when coupled with GC–MS.     

Ion-Pairing Liquid Chromatography Coupled with Mass Spectrometry for the Simultaneous Determination of Nucleosides and Nucleotides

Adenosine and its corresponding nucleotides adenosine 5'-monophosphate (AMP), adenosine 5'-diphosphate ( ADP ) and adenosine 5'-triphos-phate (ATP) are important biomolecules that provide energy and substrates for various cellular bio-chemical processes. There have been strong     

Ion-Pairing Liquid Chromatography Coupled with Mass Spectrometry for the Simultaneous Determination of Nucleosides and Nucleotides

Adenosineanditscorrespondingnucleotidesadenosine 5′monophosphate (AMP) ,adenosine 5′diphosphate (ADP)andadenosine 5′triphosphate(ATP)areimportantbiomoleculesthatprovideen ergyandsubstratesforvariouscellularbiochemicalprocesses[1] .Therehavebeenstrongde…     

Development and Validation of a RP-HPLC–PDA Method for Determination of Curcuminoids in Microemulsions

A sensitive, specific and rapid high-performance liquid chromatography method was developed in an effort to quantify extremely low curcuminoid levels for the future transdermal experiments where the curcuminoids are incorporated with excipients such as microemulsion, liposomes, and micelles. The chromatographic separation was performed using a Symmetry^® C₁₈, 250 × 4.6 mm, 5-μm column, with a mobile phase composed of 5 mM acetonitrile:phosphoric acid (45:55, v/v) at a flow rate of 1.0 mL min⁻¹, it was sensitive with a low limit of quantitation for curcuminoids (0.626 ng mL⁻¹ for curcumin) and good linearity (r ² ≥ 0.999) over the range 1–100 ng mL⁻¹. All the validation data, such as accuracy and precision, were within the required limits from the ICH guideline. The assay method was successfully applied during forced degradation of curcuminoid solutions. The method retained its accuracy and precision when the standard addition technique was applied.

     

Development and Validation of a RP-HPLC–PDA Method for Determination of Curcuminoids in Microemulsions

A sensitive, specific and rapid high-performance liquid chromatography method was developed in an effort to quantify extremely low curcuminoid levels for the future transdermal experiments where the curcuminoids are incorporated with excipients such as microemulsion, liposomes, and micelles. The chromatographic separation was performed using a Symmetry^® C₁₈, 250 × 4.6 mm, 5-μm column, with a mobile phase composed of 5 mM acetonitrile:phosphoric acid (45:55, v/v) at a flow rate of 1.0 mL min^?1, it was sensitive with a low limit of quantitation for curcuminoids (0.626 ng mL^?1 for curcumin) and good linearity (r ² ≥ 0.999) over the range 1–100 ng mL^?1. All the validation data, such as accuracy and precision, were within the required limits from the ICH guideline. The assay method was successfully applied during forced degradation of curcuminoid solutions. The method retained its accuracy and precision when the standard addition technique was applied.