Ester Hydrolysis by a Cyclodextrin Dimer Catalyst with a Tridentate N,N′,N′′‐Zinc Linking Group

A new β‐cyclodextrin dimer, 2,6‐dimethylpyridine‐bridged‐bis(6‐monoammonio‐β‐cyclodextrin) (pyridyl BisCD, L), is synthesized. Its zinc complex (ZnL) is prepared, characterized, and applied as a catalyst for diester hydrolysis. The formation constant (log K_ML=7.31±0.04) of the complex and deprotonation constant (pK_a1=8.14±0.03, pK_a2=9.24±0.01) of the coordinated water molecule were determined by a potentiometric pH titration at (25±0.1)°C, indicating a tridentate N,N′,N′′‐zinc coordination. Hydrolysis kinetics of carboxylic acid esters were determined with bis(4‐nitrophenyl)carbonate (BNPC) and 4‐nitrophenyl acetate (NA) as the substrates. The resulting hydrolysis rate constants show that ZnL has a very high rate of catalysis for BNPC hydrolysis, yielding an 8.98×10³‐fold rate enhancement over uncatalyzed hydrolysis at pH 7.00, compared to only a 71.76‐fold rate enhancement for NA hydrolysis. Hydrolysis kinetics of phosphate esters catalyzed by ZnL are also investigated using bis(4‐nitrophenyl)phosphate (BNPP) and disodium 4‐nitrophenyl phosphate (NPP) as the substrates. The initial first‐order rate constant of catalytic hydrolysis for BNPP was 1.29×10^?7 s^?1 at pH 8.5, 35 °C and 0.1 mM catalyst concentration, about 1600‐fold acceleration over uncatalyzed hydrolysis. The pH dependence of the BNPP cleavage in aqueous buffer was shown as a sigmoidal curve with an inflection point around pH 8.25, which is nearly identical to the pK_a value of the catalyst from the potentiometric titration. The k_BNPP of BNPP hydrolysis promoted by ZnL is found to be 1.68×10^?3 M ^?1 s^?1, higher than that of NPP, and comparatively higher than those promoted by its other tridentate N,N′,N′′‐zinc analogues.     

Determination of Intracellular Concentration of Acyl-Coenzyme A Esters for Metabolic Profiling Clostridium acetobutylicum

A method for determination of intracellular acyl‐coenzyme A esters in Clostridium acetobutylicum (CA) by high performance liquid chromatography (HPLC) was developed and validated. In our experiment, two important intermediates acyl‐coenzyme A esters including acetyl‐CoA, butyryl‐CoA could be baseline separated on a Zobax‐C18 column with mobile phase composed of the acetonitrile and phosphate buffer (pH 5.0). Samples treated with freeze‐thaw and protein precipitated by addition of trichloroacetic acid could be directly injected for determination of acetyl‐CoA, butyryl‐CoA with a recovery higher than 73%. With this method, the metabolite profiling of the acyl‐coenzyme A esters of CA was obtained. The comparison of the metabolite profiling between the model strain ATCC 824 and a mutant strain EA 2018, which produces higher butanol than the former was performed. Some useful information was concluded for understanding the mechanism of CA for selectively producing the solvent.     

Determination of amino acid neurotransmitters in rat hippocampi by HPLC‐UV using NBD‐F as a derivative

A simple, rapid and accurate high‐performance liquid chromatography method with ultraviolet–visible detection was developed for the determination of five amino acid neurotransmitters – aspartate, glutamic acid, glycine, taurine and γ‐aminobutyric acid – in rat hippocampi with pre‐column derivatization with 4‐fluoro‐7‐nitrobenzofurazan. Several conditions which influenced derivatization and separation, such as pH, temperature, acetonitrile percentage mobile phase and flow rate, were optimized to obtain a suitable protocol for amino acids quantification in samples. The separation of the five neurotransmitter derivatives was performed on a C₁₈ column using a mobile phase consisting of phosphate buffer (0.02 mol/L, pH 6.0)–acetonitrile (84:16, v/v) at a flow rate of 1.0 mL/min with the column temperature at 30°C. The detection wavelength was 472 nm. Without gradient elution, the five neurotransmitter derivatives were completely separated within 15 min. The linear relation was good in the range from 0.50 to 500 µmol/L, and the correlation coefficients were ≥0.999. Intra‐day precision was between 1.8 and 3.2%, and inter‐day precision was between 2.4 and 4.7%. The limits of detection (signal‐to‐noise ratio 3) were from 0.02 to 0.15 µmol/L. The established method was used to determine amino acid neurotransmitters in rat hippocampi with satisfactory recoveries varying from 94.9 to 105.2%. Copyright © 2013 John Wiley & Sons, Ltd.     

A study on the hydrolysis of bis(nitrophenyl)phosphate catalyzed by N‐methyldiethanolamine‐Ce(III) complex

The hydrolysis of bis(p‐nitrophenyl)phosphate (BNPP) catalyzed by N‐methyldiethanolamine‐Ce(III) complex in the presence and absence of cetyltrimethylammonium bromide (CTAB) and Brij35 surfactants at pH 7.20 and 303 K has been studied. The experimental results indicate that N‐methyldiethanolamine‐Ce(III) complex remarkably accelerates the hydrolysis of BNPP. The observed first‐order rate constant of the hydrolysis of BNPP catalyzed by N‐methyldiethanolamine‐Ce(III) complex at pH 7.20 and 303 K is 1.22 × 10^?2 s^?1, which is 1.09 × 10⁹ times of that of spontaneous hydrolysis of BNPP at pH 7. It is close to the activity of natural enzyme. A general quantitative treatment of the catalytic reaction involved a ternary complex as M_mL_lS has also been proposed in this paper. Applying this method to the catalytic hydrolysis of BNPP, we have obtained its thermodynamic and kinetic parameters. CTAB and Brij35 surfactant micelles obviously influence the rate constants of the catalytic hydrolysis of BNPP. Brij35 micelles promote the catalytic hydrolysis of BNPP, while CTAB micelles inhibit it. © 2004 Wiley Periodicals, Inc. Int J Chem Kinet 36: 687–692, 2004     

Studies on BNPP Cleavage by Schiff Base Complexes Containing Benzoaza‐15‐Crown‐5 in DHAB Micellar Solution

Two novel benzoaza‐crown Schiff base cobalt (II) and manganese (III) complexes were synthesized and characterized. The hydrolysis of bis(4‐nitrophenyl) phosphate (BNPP) catalyzed by the two complexes was studied in buffer solution containing dihexadecyldimethylammonium bromide (DHAB) at 25°±0.1°C and different pH values. The kinetic mathematical model of BNPP hydrolysis was proposed, and the effects of different reaction conditions on BNPP hydrolysis were discussed. The results indicate that the two complexes (MnLCl and CoL) can efficiently accelerate the catalytic cleavage of BNPP in DHAB micellar solution. The pseudo‐first‐order rate constants (k _obsd) of BNPP hydrolysis catalyzed by the metallomicelles of MnLCl/DHAB and CoL/DHAB are 2.32×10⁷ times and 1.45×10⁷ times higher than that of the BNPP spontaneous hydrolysis, respectively. Possible reasons for the huge rate accelerations include the lower critical micelle concentration (cmc) of DHAB and formation of metallomicelles made of complexes and DHAB. Furthermore, the BNPP cleavage catalyzed only by the two complexes was investigated in buffer solution. It was found that the hydrolytic rates of BNPP catalyzed only by the two complexes were about 1% of those catalyzed by MnLCl/DHAB and CoL/DHAB systems at 25°C, pH=7.00, and [BNPP]=2.0×10^?4 mol · dm^?3.     

An HPLC Method for Determination of Atropine in Human Plasma

Abstract

A development of a high performance liquid chromatographic method for the determination of atropine in human plasma is presented. Atropine is extracted from plasma basified with 0. 1N sodium hydroxide using chloroform, subsequently subjected to base hydrolysis, followed by derivatization of the generated tropic acid with 4-bromomethyl-7-methoxycoumarin (Br-Mmc). The derivative produced has a strong blue fluorescence at excitation wavelength of 328 nm and emission cutoff filter of 389 nm. d1-Mandelic acid as internal standard (I. S.) was added after hydrolysis. The chromatographic separation was achieved on a reversed phase ODS column with a mobile phase of 33% acetonitrile in 0. 01M ammonium phosphate buffer (pH 5). The minimum quantitative limit was 125 ng/ml of plasma.     

A Validated and Stability-Indicating LC Assay Method for Valdecoxib

A gradient reversed-phase liquid chromatographic assay was developed for the quantitative determination of the non-steroidal anti-inflammatory drug valdecoxib. The developed method was also applicable to the determination of related substances in the bulk drug. Forced degradation studies were performed on bulk valdecoxib using acid (2.0 N hydrochloric acid), base (2.0 N sodium hydroxide), oxidation (6.0% v/v hydrogen peroxide), water hydrolysis, heat (60 °C) and photolysis. Mild degradation was observed using alkaline conditions and considerable degradation observed during oxidative stress. Chromatographic separation of process-related impurities and degradation products was achieved using a 5 micron Zorbax SB-CN LC column. The mobile phase consisted of aqueous potassium dihydrogen phosphate (pH 3.0) and acetonitrile. Stressed samples were assayed using the developed LC method and determination of the mass balance accounted for 99.5%, thus indicating the suitability of this stability-indicating method. Linearity, accuracy, precision and robustness have also been evaluated.     

Simultaneous determination of acetylsalicylic acid and salicylic acid in human plasma by isocratic high‐pressure liquid chromatography with post‐column hydrolysis and fluorescence detection

A selective, sensitive and rapid high‐performance liquid chromatography method with post‐column hydrolysis and fluorescence detection was developed for the simultaneous quantification of acetylsalicylic acid and its metabolite salicylic acid in human plasma. Following the addition of 2‐hydroxy‐3‐methoxybenzoic acid as internal standard and simple protein precipitation with acetonitrile, the analytes were separated on a ProntoSIL 120 C₁₈ ace‐EPS column (150 × 2 mm, 3 µm) protected by a C₈ guard column (5 µm). The mobile phase, 10 mm formic acid in water (pH 2.9) and acetonitrile (70:30, v/v), was used at a flow rate of 0.35 mL/min. After on‐line post‐column hydrolysis of acetylsalicylic acid (ASA) to salicylic acid (SA) by addition of alkaline solution, the analytes were measured at 290 nm (λ_ex) and 400 nm (λ_em). The method was linear in the concentration ranges between 0.05 and 20 ng/μL for both ASA and SA with a lower limit of quantification of 25 pg/μL for SA and 50 pg/μL for ASA. The limit of detection was 15 pg/μL for SA and 32.5 pg/μL for ASA. The analysis of ASA and SA can be carried out within 8 min; therefore this method is suitable for measuring plasma concentrations of salicylates in clinical routine. Copyright © 2012 John Wiley & Sons, Ltd.     

Study on the interaction of plasma protein binding rate between edaravone and taurine in human plasma based on HPLC analysis coupled with ultrafiltration technique

In this work, two high‐performance liquid chromatography (HPLC) assays were developed and validated for the independent determination of edaravone and taurine using 3‐methyl‐1‐p‐tolyl‐5‐pyrazolone and L ‐glutamine as internal standards. In in vitro experiments, human plasma was separately spiked with a mixture of edaravone and taurine, edaravone or taurine alone. Plasma was precipitated with acetonitrile containing 0.1% formic acid. Ultrafiltration was employed to obtain the unbound ingredients of the two drugs. The factors that might influence the ultrafiltration effiency were elaborately optimized. Plasma supernatant and ultrafiltrate containing taurine were derivated with o‐phthalaldehyde and ethanethiol in the presence of 40 mmol/L sodium borate buffer (pH 10.2) at room temperature within 1 min. Chromatographic separations were achieved on an InertSustain C₁₈ column (250 × 4.6 mm, 5 µm). Isocratic 50 mmol/L ammonium acetate–acetonitrile and gradient 50 mmol/L sodium acetate (pH 5.3)–methanol were respectively selected as the mobile phase for the determination of edaravone and taurine. All of the validation data including linearity, extraction recovery, precision, accuracy and stability conformed to the requirements. Results showed that there were no significant alterations in the plasma protein binding rate of taurine and edaravone, implying that the proposed combination therapy was pharmacologically feasible. Copyright © 2014 John Wiley & Sons, Ltd.     

Development of a novel HPLC‐MS/MS method for the determination of aconitine and its application to in vitro and rat microdialysis samples

A sensitive and selective LC‐MS/MS method was developed and validated for the determination of aconitine in microdialysate and rat plasma. Extraction of plasma sample was conducted by use of 1% trichloracetic acid and acetonitrile solution with 10 ng/mL internal standard (propafenone) spiked. Microdialysates were analyzed without sample purification. After sample preparation, 2 µL were injected and separated with an isocratic mobile phase consisting of acetonitrile:0.1% formic acid (60:40, v/v) at a flow rate of 0.3 mL/min. The Agilent G6410A triple quadrupole LC/MS system was operated under the multiple‐reaction monitoring mode (MRM) using the electrospray ionization technique in positive mode. Overall, the assay exhibited good precision and accuracy. The diffusion properties of aconitine investigated in in vitro microdialysis experiments revealed unfavourable concentration dependence avertable by keeping a constant pH 5.77 using isotonic phosphate buffer solution as perfusate. The mean relative recoveries were 48.23% [coefficient of variation (CV 4.47%)] and 55.38% (CV 2.89%) for retrodialysis and recovery experiments, respectively. The in vivo recovery of aconitine was 34.48% (CV 3.05%) and was stable over the 6 h study period. Following characterization of aconitine both in vitro and in vivo microdialysis, the developed setting is suitable for application in pharmacokinetics and pharmacodynamics studies. Copyright © 2009 John Wiley & Sons, Ltd.     

Characterization of degradation products of Ivabradine by LC‐HR‐MS/MS: a typical case of exhibition of different degradation behaviour in HCl and H2SO4 acid hydrolysis

A validated stability‐indicating HPLC method was established, and comprehensive stress testing of ivabradine, a cardiotonic drug, was carried out as per ICH guidelines. Ivabradine was subjected to acidic, basic and neutral hydrolysis, oxidation, photolysis and thermal stress conditions, and the resulting degradation products were investigated by LC‐PDA and LC‐HR‐MS/MS. The drug was found to degrade in acid and base hydrolysis. An efficient and selective stability assay method was developed on Phenomenex Luna C18 (250 × 4.6 mm, 5.0 µm) column using ammonium formate (10 mM, pH 3.0) and acetonitrile as mobile phase at 30 °C in gradient elution mode. The flow rate was 0.7 ml/min and detection wavelength was 286 nm. A total of five degradation products (I‐1 to I‐5) were identified and characterized by LC‐HR‐MS/MS in combination with accurate mass measurements. The drug exhibited different degradation behaviour in HCl and H₂SO₄ hydrolysis conditions. It is a unique example where two of the five degradation products in HCl hydrolysis were absent in H₂SO₄ acid hydrolysis. The present study provides guidance to revise the stress test for the determination of inherent stability of drugs containing lactam moiety under hydrolytic conditions. Most probable mechanisms for the formation of degradation products have been proposed on the basis of a comparison of the fragmentation pattern of the drug and its degradation products. In silico toxicity revealed that the degradation products ( I‐2 to I‐5 ) were found to be severe irritants in case of ocular irritancy. The analytical assay method was validated with respect to specificity, linearity, range, precision, accuracy and robustness. Copyright © 2015 John Wiley & Sons, Ltd.     

Enantiomeric separation of 2‐arylpropionic acid nonsteroidal anti‐inflammatory drugs by HPLC with hydroxypropyl‐β‐cyclodextrin as chiral mobile phase additive

The enantio‐separations of eight 2‐arylpropionic acid nonsteroidal anti‐inflammatory drugs (2‐APA NSAIDs) were established using reversed‐phase high‐performance liquid chromatography with hydroxypropyl‐β‐cyclodextrin (HP‐β‐CD) as chiral mobile phase additive for studying the stereoselective skin permeation of suprofen, ketoprofen, naproxen, indoprofen, fenoprofen, furbiprofen, ibuprofen and carprofen. The effects of the mobile phase composition, concentration of HP‐β‐CD and column temperature on retention and enantioselective separation were investigated. With 2‐APA NSAIDs as acidic analytes, the retention times and resolutions of the enantiomers were strongly related to the pH of the mobile phase. In addition, both the concentration of HP‐β‐CD and temperature had a great effect on retention time, but only a slight or almost no effect on resolutions of the analytes. Enantioseparations were achieved on a Shimpack CLC‐ODS (150 × 4.6 mm i.d., 5 μm) column. The mobile phase was a mixture of methanol and phosphate buffer (pH 4.0–5.5, 20 mM) containing 25 mM HP‐β‐CD. This method was flexible, simple and economically advantageous over the use of chiral stationary phase, and was successfully applied to the enantioselective determination of the racemic 2‐APA NSAIDs in an enantioselective skin permeation study. Copyright © 2009 John Wiley & Sons, Ltd.     

Selective determination of famotidine in human plasma by high performance liquid chromatography in alkaline media with solid phase extraction

A new method is described for the determination of famotidine by solid phase extraction from alkalinized human plasma followed by reversed phase (RP) HPLC in acetonitrile/alkaline buffer with molsidomine as an internal standard. Different acetonitrile/aqueous buffer mobile phases as well as various RP columns were used. Alkaline medium allowed the limit of quantitation to be lowered to 5 ng/mL of plasma as the famotidine gives more intense absorption at about 286 nm (at pH values higher than 7). Moreover, work in alkaline media and at this wavelength is highly selective as peaks corresponding to impurities present in most samples are well separated. A method using a mildly alkaline mobile phase (acetonitrile/10 mM phosphate with 10 mM 1‐heptanesulphonic acid, pH 7.5) was successfully used for determination of famotidine in human plasma in a pharmacokinetic study.     

Precise synthesis of pH‐responsive copolymers with naphthoic acid side groups via living cationic polymerization

pH‐Responsive homopolymers and copolymers with naphthoic acid side groups were synthesized via base‐assisting living cationic polymerization. To this end, the feasibility of the living cationic polymerization of ethyl 6‐[2‐(vinyloxy)ethoxy]‐2‐naphthoate (EVEN) was first examined using a base‐assisting initiating system. Et_1.5AlCl_1.5 as a Lewis acid catalyst induced the living cationic polymerization of EVEN in the presence of ethyl acetate or 1,4‐dioxane in CH₂Cl₂ at 0 °C. In contrast, the use of naphthoxyethyl vinyl ether (NpOVE), which is a nonsubstituted counterpart, resulted in a poorly controlled polymerization under these conditions. The presence of the carboxy ester was most likely critical in preventing side reactions. A subsequent alkaline hydrolysis of the side‐chain esters quantitatively yielded a carboxy‐containing polymer. Aqueous solutions of this polymer underwent pH‐driven phase separation at pH 7.0. Well‐defined random and block copolymers were also prepared with various functional segments, and their stimuli‐responsive behaviors were investigated in terms of solution transmittance and aggregate size. Block copolymers containing two different pH‐responsive segments formed micelle‐like structures between the two phase‐separated pH values, and dual stimuli‐responsive copolymers containing a pH‐responsive polyacid segment and a thermosensitive segment self‐assembled in the water in response to both the pH and temperature. © 2013 Wiley Periodicals, Inc. J. Polym. Sci., Part A: Polym. Chem. 2013 , 51, 5239–5247     

Electrochemical Determination of Synephrine by Hydrophilic Interaction Liquid Chromatography Using a Zwitterionic Monolith Column

A sensitive method for the electrochemical determination of synephrine (SYN) by hydrophilic interaction liquid chromatography (HILIC) has been developed. Optimal chromatographic separation and high sensitive determination by HILIC with electrochemical detection (HILIC‐ECD) was achieved using a sulfobetaine‐type zwitterionic monolith column (100×1.02 mm, i.d.), a mixture of 10 mM sodium phosphate (pH 4) and acetonitrile (20 : 80, v/v) as mobile phase, and a glassy carbon working electrode which was applied with a potential at +1.0 V vs. Ag/AgCl. The chromatographic peak height of SYN was proportional to the concentration from 5.0 µg/L to 1.0 mg/L (r=0.999). The detection limit of SYN (S/N=3) was 3.7 pg on the column. Moreover, the present HILIC‐ECD could be applied to the accurate and precise determination of SYN in Aurantii nobilis Pericarpium. In conclusion, we have demonstrated that an ECD is one of useful detection methods applicable to HILIC.     

Electropolymerization of Thin Film Conducting Polymer and Its Application for Simultaneous Determination of Ascorbic Acid,Dopamine and Uric Acid

In this paper electropolymerization of a thin film of para‐phenylenediamine (PPD) is studied at glassy carbon electrode (GCE) in sulfuric acid media by cyclic voltammetry. The results showed that this polymer was conducting and had a reproducible redox couple in the potential region from 0.0 to 0.4 V in phosphate buffer solution. This modified GCE (p‐PPD‐GCE) was applied for simultaneous determination of ascorbic acid (AA), dopamine (DA) and uric acid (UA) using differential pulse voltammetry (DPV). The p‐PPD‐GCE in 0.1 M phosphate buffer solution (pH 5.0) separated the DPV signals of AA, DA and UA with sufficient potential differences between AA–DA and DA–UA and also enhanced their oxidation peak currents. The oxidation currents were increased from 2.0 to 2000.0 µM for AA, 10.0 to 1250.0 µM for DA and 50.0 to 1600.0 µM for UA. The detection limits were evaluated as 0.4, 1.0 and 2.5 µM for AA, DA and UA, respectively (S/N=3).     

Resolving the enigma of prebiotic C?O?P bond formation: Prebiotic hydrothermal synthesis of important biological phosphate esters

Important biological phosphate esters such as sn‐glycerol‐3‐phosphate, glycerol‐2‐phosphate, and phosphoethanolamine were synthesized under hydrothermal conditions. Phosphorus was incorporated into the biomolecules, leading to the formation of C O P type compounds hydrothermally. Only perlite‐catalyzed reaction at 180°C could result in the formation of sn‐glycerol‐3‐phosphate, whereas glycerol‐2‐phosphate could be easily synthesized at 100°C with or without minerals and phosphoethanolamine was obtained within a temperature range of 100 to 120°C. © 2010 Wiley Periodicals, Inc. Heteroatom Chem 21:161–167, 2010; Published online in Wiley InterScience ( www.interscience.wiley.com ). DOI 10.1002/hc.20591     

A Stability-Indicating LC Method for Candesartan Cilexetil

An isocratic reversed-phase liquid chromatographic method has been developed for quantitative determination of candesartan cilexetil, used to treat hypertension, in the bulk drug and in pharmaceutical dosage forms. The method is also applicable to analysis of related substances. Chromatographic separation was achieved on a 250 mm × 4.6 mm, 5 μm particle, CN column with a 50:50 (v/v) mixture of phosphate buffer, pH 3.0, and acetonitrile as mobile phase. The flow rate was 1.0 mL min⁻¹ and the detection wavelength was 210 nm. Resolution of candesartan cilexetil and six potential impurities was greater than 2.0 for all pairs of compounds. The drug was subjected to hydrolytic, oxidative, photolytic, and thermal stress and substantial degradation occurred in alkaline and acidic media and under oxidative and hydrolytic stress conditions. The major product obtained as a result of basic hydrolysis was different from that produced by acid hydrolysis and aqueous hydrolysis. The stress samples were assayed against a reference standard and the mass balance was found to be close to 99.6%. The method was validated for linearity, accuracy, precision, and robustness.     

Synthesis of novel ladder polymers of poly(3,4‐dihydro‐2H‐pyran‐2‐methanol)

Polydi(3,4‐dihydro‐2H‐pyran‐2‐methyl) esters of oxalic, adipic, and phthalic acids were prepared at different temperatures in the presence of different cationic initiators, namely, the boron trifluoride/diethyl ether complex system, anhydrous ferric chloride, and p‐toluene sulfonic acid. The obtained polymers were hydrolyzed under basic conditions, and the polydispersity indices of these polymers were determined before and after hydrolysis. The results are discussed to shed some light on the ability to use this analysis to investigate the precise structure of the obtained polymers and to predict the ability of these polymers to form ladder or semiladder polymers. Characteristics of such polymers were dependent, to some extent, on the type of crosslinks and the cationic initiators used for polymerization as well as the reaction temperature. It seems possible to optimize the conditions leading to formation of ladder or semiladder polydi(3,4‐dihydro‐2H‐pyran‐2‐methyl) esters of oxalic acid and adipic acid, respectively. The ladder structure was confirmed through determination of the polydispersity index before and after hydrolysis of the polymer formed at different temperatures and through computer‐aided molecular modeling. © 2002 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 40: 3909–3915, 2002     

New Validated Methods for the Simultaneous Determination of Two Multicomponent Mixtures Containing Guaiphenesin in Syrup by HPLC and Chemometrics‐Assisted UV‐Spectroscopy

Abstract

High pressure liquid chromatographic (HPLC) and spectrophotometric methods are developed for the determination of two multicomponent mixtures containing guaiphenesin, dextromethorphane hydrobromide, and sodium benzoate together with either phenylephrine hydrochloride, chlorpheniramine maleate, and butylparaben (mixture 1) or ephedrine hydrochloride and diphenhydramine hydrochloride (mixture 2). The HPLC method depended on using an ODS column with mobile phase consisting of acetonitrile ?10 mM potassium dihydrogen phosphate, pH 2.7 (40∶60 v/v) containing 5 mM heptane sulfonic acid sodium salt (for mix 1) and a cyanopropyl column with mobile phase consisting of acetonitrile ?12 mM ammonium acetate, pH 5 (40∶60 v/v) (for mix 2) and UV detection at 214 nm. The cyanopropyl column is much less hydrophobic, less sterically restricted to the penetration of bulky solute molecules into the stationary phase, and has weaker hydrogen‐bond acidity than the ODS column. So the cyanopropyl column is more suitable for separation of components of mix 2. The chemometric‐assisted spectrophotometric method with, principal component regression (PCR) and partial least squares (PLS‐1) was used. For the chemometric method a calibration 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 in the spectral region (210–240 or 210–224 nm for mix 1 and mix 2, respectively, as this range provided the greatest amount of information about the two mixture components). The spectrophotometric method does not require a separation step. The proposed methods were successfully applied for the analysis of the two multicomponents combinations in laboratory‐prepared mixtures and in commercial syrups, and the results were compared with each other.