Int J Pharm Pharm Sci, Vol 6, Issue 10, ??-??Original Article

HPLC METHOD DEVELOPMENT AND VALIDATION: SIMULTANEOUS DETERMINATION OF ACTIVE INGREDIENTS IN COUGH AND COLD PHARMACEUTICALS

HATİCE ÇAĞLAR, EBRU BÜYÜKTUNCEL

Inonu University, Faculty of Pharmacy, Department of Analytical Chemistry, 44280 Malatya, Turkey.
Email: saliha.buyuktuncel@inonu.edu.tr

Received: 07 Sep 2014 Revised and Accepted: 03 Oct 2014

ABSTRACT

Objective: This study aimed to develope a simple reversed-phase high performance chromatographic method for simultaneous determination of pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr, diphenhydramine HCI in cough and cold pharmaceuticals.

Methods: The separation of these compounds was achieved within 37.9 min on a Nucleodur gravity C18 column (250 x 4.0 mm, 5μm). The chromatographic separation of these compounds performed in a single run by using isocratic mobile phase consisting of methanol:buffer mixture (38:62, v/v) at room temperature, with flow rate of 0.75 mL.min-1.

An ultraviolet absorption at 210 nm was monitored. 2,4,6-trimethoxybenzaldehyde was used as an internal standard (ISTD). The selectivity, linearity of calibration, accuracy, intraday and interday precision and forced degradation studies were examined as parts of the method validation.

Results: The concentration–response relationship was linear over a concentration range of 0.2-250 µg.mL-1 for acetaminophen, 0.5–250 µg.mL-1 for pseudoephdrine HCI and pheniramine maleate, 1–250 µg.mL-1 for guaifenisin, 2.5-250 µg.mL-1 for chlorpheniramine maleate and triprolidine HCI, 5-250 µg.mL-1 for pyrilamine maleate and diphenhydramine HCI, 10-20 µg.mL-1 for dextromethorphan HBr with correlation coefficients better than 0.9993. The relative standard deviations of the intraday and interday were all less than 4%. Conclusion: The proposed liquid chromatographic method was successfully applied for the routine analysis of these compounds in different cough and cold pharmaceutical preparations such as syrups and tablets.

Keywords: High performance liquid chromatography, Active Ingredients Cough and Cold Pharmaceuticals, Validation.

INTRODUCTION

Cough and cold pharmaceutical preparations are one of the most extended formulations in the world and have got many pharmaceutical forms: syrup, suspension, sachets, capsules and tablets [1]. These preparations represent complex formulations containing several active ingredients and a broad spectrum of excipients such as flavoring agents, saccharose or aspartame, acidulants, natural or artificial colorings and flavoring agents, dyes sweeteners and preservatives [2,3]. These compounds are contained in the pharmaceutical form in very different proportions and present chemical forms of very different nature [4].

Acetaminophen (paracetamol) is analgesic and antipiretic [5]. As pain and fever are common, no home should be without some paracetamol, particularly homes with children. Acetaminophen is available in many different pharmaceutical preparations such as tablets, capsules, and liquid suspensions [6]. Chlorpheniramine maleate inhibits the effects of histamine on capillary permeability and bronchial smooth muscles. It is an anti-allergic drug, widely used in cough-cold preparations. The combination of antihistamine such as pyrilamine maleate and chlorpheniramine maleate is used to overcome the allergic effects and reduce or relieve cold symptoms [3]. Pheniramine maleate, dipenhydramine HCI, triprolidine HCI and pseudoephedrine hydrochloride are widely used in combination with other drugs for the clinical treatment of common cold, sinusitis, bronchitis and respiratory allergies [7]. Two common actives in such products are dextromethorphan HBr and guaifenesin. Dextromethorphan HBr is an antitussive which acts through depression of the medullary centers of the brain to decrease the involuntary urge to cough [8-11]. Guaifenesin is an expectorant believed to stimulate receptors that initiate a reflex secretion of respiratory tract fluid, thereby increasing the volume while decreasing the viscosity of mucus in the lungs. This action facilitates removal of mucus and reduces irritation of the bronchial tissue. Dextromethorphan hydrobromide and guaifenisin were used as cough suppressants antitussive for the relief of nonproductive cough and cold preparations [12]. All these components have different polarities and exist in very different proportion. Due to these characteristics and because of diverse properties inherent to their formulation, these preparations offer an analytical problem [13].

A variety of methods exist in the literature for the determination of some of these compounds [6,14-23]. Among them Louhaichi et al., have provided maximum separation that six active ingredients were separated, simultaneously [23]. But the presented study has identified the separation of nine active ingredients simultaneously.

The aim of this study was to develop basic, accurate and selective LC method for the simultaneous determination of pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr, diphenhydramine HCI in cough and cold pharmaceuticals. The method was then subjected to validation. The validation characteristics were evaluated as the selectivity, intraday and interday precision, linearity, accuracy, LOQ and LOD values and stress forced degradation studies.

The proposed liquid chromatographic method was successfully applied for the routine analysis of these compounds in different cough and cold pharmaceutical preparations such as syrups and tablets.

MATERIALS AND METHODS

Instrumentation and Chromatographic Conditions

The integrated high performance liquid chromatography system (LC 1100, Hewlett-Packard, USA) is equipped with a diode-array UV detector, a quarternary pump, a degasser, an autosampler, an injector with 20 µL loop, and a column oven. Different columns were tested for analysis and pseudoephedrine HCI and acetaminophen peaks was observed to overlap in the other columns. Therefore separation was carried out using Nucleodur gravity C18 column (250 x 4.0 mm, 5μm).

The mobile phase was a mixture of 38% methanol, 62% of 80 mM KH2PO4 aqueous solution adjusted to pH 3.0, to which was added 10% (v/v) orthophosphoric acid. The mobile phase was vacuum-filtered through a 0.45 μm nylon filter and degassed on-line by micro vacuum degasser. The chromatographic separation of these compounds performed at room temperature. Analysis was run at flow rate of 0.75 mL.min-1 with 37.9 min run time. The analysis was carried out at 210, 220, 254 and 280 nm and the best separation and high peak area have been monitored at 210 nm. The injection volume was 20 μL.

Reagents and Chemicals

Pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr, diphenhydramine HCI, HPLC grade methanol, sodium benzoate, 1,2-propylene glycol, citric acid, sorbitol and sodium saccharin were purchased from Sigma-Aldrich. Sodium carboxymethyl cellulose, pseudoephdrine HCI, 2,4,6-trimethoxybenzaldehyde, sunset yellow, and orthophosphoric acid were purchased from Fluka. Potassium dihydrogenphosphate and glycerol were obtained from Riedel-de Haën. Orange and cinnamon flavor were purchased from Eurofragance.

Water was purified (18 MΩ cm−1 quality) from New Human Power I (Korea).

The commercialized pharmaceutical products used are detailed below:

Actidem syrup (10 mg dextromethorphan HBr, 30 mg pseudoephedrine HCI and 1.25 mg/5 mL triprolidine HCI for 150 mL) was manufactured by GlaxoSmithKline, France.

Actifed syrup (30 mg pseudoephedrine HCI and triprolidine HCI 1.25 mg/5 mL for 150 mL) was manufactured by GlaxoSmithKline, France.

Aferin plus pediatric syrup (160 mg acetaminophen, 1 mg chlorpheniramine maleate, 15 mg/5 mL for 100 mL) was manufactured by Hüsnü Arsan, Turkey.

Benical syrup (10 mg dextromethorphan HBr, 20 mg pseudoephedrine HCI, 2 mg/5 mLchlorpheniramine maleate for 100 mL) was manufactured by Bayer, Germany.

Corsal syrup (120 mg acetaminophen, 2 mg chlorpheniramine maleate, 5 mg/5 mL phenylephrine HCI for 120 mL) was manufactured by İ.E Ulagay, Turkey.

Katarin pediatric syrup (120 mg acetaminophen, 50 mg oxolamine citrate, 1 mg/5 mL chlorpheniramine maleate for 100 mL) was manufactured by Biofarma, Turkey.

Kongest syrup (160 mg acetaminophen, 2.5 mg chlorpheniramine maleate, 1 mg/5 mL phenylephrine HCI for 100 mL) was manufactured by Eczacıbaşı, Turkey.

Peditus syrup (120 mg acetaminophen, 50 mg guaifenesin, 6.25 mg pyrilamine maleate, 5 mg/5 mL phenylephrine HCI for 100 mL) was manufactured by Sandoz, Turkey.

Sudafed syrup (30 mg/5 mL pseudoephedrine HCI for 150 mL) was manufactured by GlaxoSmithKline, France.

Benical cold film tablet (500 mg acetaminophen, 30 mg pseudoephedrine HCI, 20 mg dextromethorphan HBr for one tablet) was manufactured by Bayer, Germany.

Corsal capsule (300 mg acetaminophen, 2 mg chlorpheniramine maleate, 5 mg phenylephrine HCI for one tablet) was manufactured by İ.E Ulagay, Turkey.

Gerakon fort tablet (650 mg acetaminophen, 10 mg phenylephrine HCI, 4 mg chlorpheniramine maleate for one tablet) was manufactured by Münir Şahin, Turkey.

Kongest forte tablet (650 mg acetaminophen, 4 mg chlorpheniramine maleate, 10 mg phenylephrine HCI for one tablet) was manufactured by Eczacıbaşı, Turkey.

Sudafed syrup (60 mg pseudoephedrine HCI for one tablet) was manufactured by GlaxoSmithKline, France.

Theraflu forte film tablet (650 mg acetaminophen, 10 mg phenylephrine HCI, 4 mg chlorpheniramine maleate for one tablet) was manufactured by Novartis, Switzerland.

All these medicines were purchased by local pharmacy.

Standard solutions and sample preparation for quantification

Stock standard solutions of pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr and diphenhydramine HCI were prepared in ultrapure water. The calibration curves were prepared by diluting the stock solution in the mobile phase to furnish solutions with final concentrations of 0.2-250 µg.mL-1 for acetaminophen, 0.5–250 µg.mL-1 for pseudoephdrine HCI and pheniramine maleate, 1–250 µg.mL-1 for guaifenisin, 2.5-250 µg.mL-1 for chlorpheniramine maleate and triprolidine HCI, 5-250 µg.mL-1 for pyrilamine maleate and diphenhydramine HCI, 10-250 µg.mL-1 for dextromethorphan HBr.

The syrup placebo was prepared wherein: Citric acid was dissolved in glycerin. Sodium benzoat, sorbitol and sodium saccharin were dissolved in ultra pure water. Sodium carboxymethyl cellulose was kept in water for swelling. Then propylene glycol, flavors and colouring agent were added to this mixture and diluted with ultrapure water to 100 mL [24]. The excipients of syrup placebo were shown in Table 1.

Table 1: Excipients of placebo syrup

Excipients Amount
Citric Acid 0.3 g
Glycerin 10 g
Propylene glycol 10 g
Sodium benzoat 0.02 g
Sodium carboxymethyl cellulose 0.1 g
Sorbitol 20 g
Sodium saccharin 0.04 g
Sunset yellow enough amount
Orange aroma 1 drop
Cinnamon aroma 1 drop

The amounts of the commercial cough and cold liquid were depending on the drug concentration of various products. The commercial cough and cold syrups were diluted with mobile phase according to linear range of standards. The resulting solutions were vortexed for 15 min and a portion of the sample was filtered through a 0.45 µm filter before injection in the HPLC.

The mean weight of finely powdered tablets were accurately transferred into 50 mL calibrated flask and ultrapure water was added. The mixtures were extracted in the ultrasonic bath for 15 min at room temperature and diluted with ultrapure water to the mark. The solutions were filtered through a 0.45 µm filter. Then the solutions were diluted with mobile phase depending on the drug concentration of various products. All preparations were performed in three replicates.

System Suitability Tests

As system suitability test is an integral part of chromatographic methods development and it is used to verify that the system is adequate for the analysis to be performed, the parameters for pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr and diphenhydramine HCI were evaluated. Several parameters may be used to demonstrate that the chromatographic system as a whole continues to be fit for the intended purpose. As well as monitoring the column performance, we can monitor the performance of the injector, pumps, and detector and so together provide an overview of system suitability. The user may define the minimum performance values or acceptance criteria according to local needs or business requirements [25].

System suitability test parameters were checked to ensure that the system was working correctly during the analysis [26]. Parameters which are typically used in suitability evaluations are capacity factor (k’), selectivity factor (α), resolution (R), number of theoretical plates (N) and tailing factor (T). For an optimum separation, capacity factor should be in the range of 0.5 < k’ <10. A value of 1.5 for resolution implies a complete separation of two compounds. The number of theoretical plates must be higher than 2000. The calculated values of tailing factor should be in the range of 0.5 ≤ T ≤ 2.

Validation

A full validation of assay consisting of selectivity, linearity, lower limit of detection and quantitation (LOD and LOQ), intraday and interday accuracy and precision of the method was performed according to the ICH description [27].

Selectivity

Selectivity is the ability to assess unequivocally the analyte in the presence of components which may be expected to be present.

Linearity and Range

The linearity of the assay was performed with a six point calibration curve prepared by diluting stock analyte solution in placebo syrup sample for five consecutive days. Six point calibration curves of each analyte were obtained by linear regression analysis.

The lowest concentration that can be quantified (LOQ) with acceptable accuracy and precision was evaluated at a signal-to-noise ratio of 10. Limit of detection (LOD) was evaluated at a signal-to-noise ratio of 3.

Accuracy and Precision

The accuracy of the proposed procedure was evaluated by means of recovery experiments. Recoveries were calculated as peak area ratios of reference standard/analyte (spiked placebo) at different concentration.

The precision was expressed as relative standard deviation of a series of measurements. Three different concentrations of standard solutions were analyzed five consecutive days and five times within the same day.

Forced Degradation Conditions

Forced degradation studies was carried out to demonstrate that the method was stability indicating. Solutions were prepared containing each substance at working standard concentration. They were treated with the following conditions:

a) Acid conditions: Solutions were acidulated with 37% HCl to reach a final concentration of 0.1 M HCl and heated for 2 h and 8 h at 80ºC, respectively.

b) Basic conditions: Solutions were treated with 1 M NaOH to reach a final concentration of 0.1 M NaOH and heated for 2 h and 8 h at 80ºC, respectively.

c) Oxidation with H2O2: Solutions were treated with 3% (v/v) H2O2 for 2 h and 8 h, respectively.

d) UV radiation: Solutions were exposed under a UV light at 254 nm during 35 h.

e) Thermal conditions: Solutions were heated for 2 h, 8 h and 24 h at 60 ºC and 80 ºC, respectively.

RESULTS AND DISCUSSION

Method Optimization

The first step of the study was the optimization of the chromatographic conditions. Various mobile phase combinations were tried initially to separate pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr and diphenhydramine HCI on C18 column. The mixture of methanol and phosphate buffer (38:62, v/v) was capable of a good separation and sensitivity (Figure1).

Fig. 1: Effect of methanol and phosphate buffer composition on separation of the mixture

The effect of phosphate buffer concentration (20, 40, 60, 80 ve 100 mM ) on the retention time of mixture was investigated in methanol-buffer (38:62) mobile phase. The concentration of the phosphate buffer solution was chosen as 80 mM for optimum separation (Figure 2).

Fig. 2: Effect of phosphate buffer concentration on separation of the mixture.

In order to find suitable buffer pH, the effect of pH on retention and resolution was investigated over the range of 2.0 and 6.0, using 10% (v/v) ortho-phosphoric acid solution. pKa values of these compounds are higher than 8. The changes in retention time as a function of pH result from changes in the ionization form of these solutes. Therefore, a pH value of 3.0 was selected because of optimum resolution. As shown in Figure 3, the resolution of all active compounds under the optimum conditions was adequate.

Fig. 3: Effect of phosphate buffer pH on separation of the mixture


Fig. 4: A typical chromatogram of standard active ingredients. 1, maleic acid; 2, acetaminophen; 3, pseudoephedrine HCI; 4, pheniramine maleate; 5, guaifenisin; 6, pyrilamine maleate; 7, 2,4,6-trimethoxybenzaldehyde; 8, chlorpheniramine maleate; 9, triprolidine HCI; 10, dextromethorphan HBr; 11, diphenhydramine HCI.

Method Validation

System suitability

The important parameter t0 was 2.319± 0.062 min in the analysis. This was the time of KBr peak. The capacity factor (k') values were in the range of 0.5 < k’ <10 except dextromethorphan HBr and diphenhydramine HCI. The resolution value for separation of acetaminophen and pseudoephedrine HCI was 1.3801 and dextromethorphan HBr and diphenhydramine HCI was 1.4995. The resolution values of other compounds were higher than 1.5. The therotical plate numbers of all compounds were higher than 2600 and the calculated tailing factors of them were obtained in the acceptable range of 0.5 ≤ T ≤ 2.

Selectivity

The representive chromatogram (Figure 5) of placebo solution constituted by excipient blend showed that there was no interfering peak in the retention times corresponding to the analytes. Therefore, the proposed method was considered to be selective.

Fig. 5: Chromatogram of placebo solution, 1. citric acid; 2. sodium benzoate.

Linearity and Range

To evaluate linearity of the method, six different concentrations of the nine analytes in the range of 0.2-250 mg mL-1 for acetaminophen, 0.5-250 mg mL-1 for pseudoephedrine HCI and pheniramine maleate, 1-250 mg mL-1 for guaifenisin, 5-250 mg mL-1 for pyrilamine maleate and diphenhydramine HCI, 2.5-250 mg mL-1 for chlorpheniramine maleate and triprolidine HCI, 10-250 mg mL-1for dextromethorphan HBr were analysed and the calibration curves for nine active compounds constructed under optimum conditions as the ratio of the peak areas of analysed subtance to internal standard against the concentration and the results are presented in Table 2.

The limit of detection (LOD) and limit of quantification (LOQ) of the method were determined by injecting progressively low concentrations of the standard solutions.

Accuracy and Precision

Accuracy was evaluated with recoveries obtained in the analysis of synthetic sample prepared in the placebo and compared with the corresponding standards. The results indicate good accuracy of the method for the simultaneous determination of the active compounds as revealed by mean recovery data. The results are given in Table 3. For evaluation of the precision estimates, intra-day and inter-day precision were performed for each active compound. The intra-day precision of the method was determined by preparing the standards of nine active compounds at three different concentration and values for each compounds were determined by five repeated analyses. Inter-day precision was check with the same concentration as intra-day assay, and the determination of each active compound was repeated day by day during five days. The obtained results are shown in Table 3.

Table 2: Linearity study results (n=5)

Acetaminophen Psudoephedrine HCI Pheniramine

Maleate

 Guaifenis in Pyrilamine

Maleate

 Chlorpheniramine Maleate Triprolidine HCI Dextromethorphan HBr Diphenhydramine HCI Acetaminophen
Regression

equation

 y=0.3659x+0.0583 y=0.3x+0.0134 y=0.3698x-0.0462 y=0.2798x+0.0225 y=0.2236x-0.0015 y=0.3101x-0.0205 y=0.4438x+0.0116 y=0.2556x-0.0351 y=0.4565x-0.0059
Standard error of intercept 0.0222 0.0047 0.0188 0.0175 0.0011 0.0092 0.0162 0.0046 0.0243
Standard error of slope 0.0244 0.0071 0.0099 0.0162 0.0012 0.0085 0.0058 0.0007 0.0091
Correlation coefficient (r) 0.9993 0.9997 0.9993 0.9991 0.9999 0.9999 0.9998 0.9990 0.9997
Linearity range (mg L-1) 0.2-250 0.5-250 0.5-250 1-250 5-250 2.5-250 2.5-250 10-250 5-250
LOD (mg L-1) 0.1 0.1 0.2 0.2 0.2 0.5 0.75 2.5 0.75
LOQ (mg L-1) 0.3 0.5 0.75 1 5 2.5 2.5 10 5

Forced Degradation

The drug substances was found almost stable in peroxide degradation. No degradation was seen in 3% H2O2 at 80 °C up to 2 and 8 hours.

Under the acidic conditional at the end of 2h and 8 h, large amount of fall in active compounds peaks area was observed except guaifenisin.

Under the alkaline conditional at the end of 8 h, same active compounds peaks was disappeared.

For photo degradation studies, all standards solution exposed to UV-light for 35 h: in these condition no a large amount of fall in peaks area.

For thermal degradation studies, all standard solutions were heated for 2 h and 8 h at 60 ºC and 80 ºC, respectively: in these condition no a large amount of fall in peaks area.

The all results were given Table 4.

Analysis of samples

Chromatograms of the some samples were shown below (Fig.6-12). The amount of each active compound was appointed using calibration curve method. The results demonstrate that the label claims of drugs close with obtained results which confirms the good accuracy of the proposed method (Table 5, Table 6).

Table 3: The intra-assay (intra-day) and between-assay (inter-day) precision and accuracy results (n=5)

  Intra-day Inter-day
Compound Added
(mg L-1)		 Precision
(RSD%)		 Accuracy
(Recovery%)		 Precision
(RSD%)		 Accuracy
(Recovery%)
Acetaminophen 50 1.4420 101.6520 1.4658 101.9980
100 0.6876 100.3878 0.6902 101.2141
250 1.0201 100.5995 1.1025 102.3410
Pseudoephedrine
HCI		 50 3.3608 98.7927 3.7541 96.3060
100 1.3449 100.0609 1.3457 100.2120
250 0.3759 99.9519 0.3854 100.5387
Pheniramine
Maleate		 50 2.3691 99.1892 2.3499 100.1165
100 1.2286 101.1458 1.2427 103.1933
250 1.0122 99.4358 1.0065 100.0570
Guaifenisin 50 0.9491 100.8194 0.9569 101.0235
100 0.7833 100.2711 0.7854 100.3749
250 2.2236 101.6682 2.5607 103.1516
Pyrilamine
Maleate		 50 3.9870 101.2402 4.0364 103.0688
100 3.3658 100.8789 3.3954 101.0122
250 3.9282 99.0023 3.8890 100.0521
Chlorpheniramine
Maleate		 50 2.5739 101.8374 2.6212 102.056
100 0.5632 100.9189 0.5684 100.9465
250 1.4962 101.3465 1.5163 102.9471
Tripirolidine HCI 50 2.2186 100.0368 2.9564 101.5857
100 1.6736 102.1042 1.7089 103.2254
250 2.0286 101.1976 2.6815 103.8761
Dextromethorphan
HBr		 50 2.0466 99.5917 2.9157 102.0081
100 2.0346 101.4256 2.0636 101.9875
250 1.2113 100.8714 1.2218 101.0159
Diphenhydramine
HCI		 50 1.1565 100.6600 1.1641 101.1572
100 0.4162 100.2087 0.4170 100.8704
250 0.4766 99.4162 0.4738 99.9141

Table 4: The results of stress tests

  HCIb H2O2b NaOHb  Photolitic Thermal Degradation b
2 h 80 ºC 8 h 80 °C 2 h 80 °C 8 h 80 °C 2 h 80 °C 8 h 80 °C  UV Lamp
35 h 2 h 60 °C 8 h 60 °C 24 h 60 °C 2 h 80 °C 8 h 80°C 24 h 80 °C
Acetaminophen 56.12 0 99.5 86.3 53.8 0  94.5 99.1 98.6 98.7 98.9 96.6 9\=7.3
Pseudoephedrine HCI 73.07 65.8 97.3 95.6 80.5 74.6  91.1 98.9 97.3 96.9 98.3 96.5 95.9
Pheniramine Maleate Poor peak shape Poor peak
shape		 93.1 84.3 70.9 57.2  72.7 96.5 95.7 89.1 94.1 88.2 85.4
Guaifenisin 94.1 91.9 98.2 95.7 83.5 63.8  90.5 99.8 99.2 98.6 99.3 98.9 98.0
Pyrilamine Maleate 76.7 36.3 89.9 86.2 46.8 0  74.4 96.8 95.2 89.7 89.2 85.9 82.9
Chlorpheniramine
Maleate		 90.4 78.2 94.7 75.9 54.9 20.9  54.3 95.8 94.3 90.1 93.5 90.5 87.3
Triprolidine HCI 81.1 71.7 90.4 79.4 23.3 0  82.0 95.1 93.0 89.4 92.4 88.7 85.8
Dextromethorphan HBr 84.7 63.9 98.8 92.7 93.0 36.4  71.5 99.2 98.5 96.5 98.8 96.1 92.7
Diphenhydramine HCI 18.9 6.6 97.5 85.9 30.3 0  72.5 99.5 97.6 88.7 98.6 90.8 87.2

aRecovery(%) =[(mg.mL-1) after stres/(mg.mL-1) initial analyze]x100, bStress conditions


Fig. 6: The chromatogram belongs to corsal syrup, 1, acetaminophen; 2, sodium benzoate; 3, ISTD; 4, chlorpheniramine maleate.


Fig. 7: The chromatogram belongs to actidem syrup, 1, pseudoephedrine HCI; 2, sodium benzoate; 3, ISTD; 4, triprolidine HCI; 5, dextromethorphan HBr.


Fig. 8: The chromatogram belongs to actifed syrup, 1, pseudoephedrine HCI; 2, sodium benzoate; 3, ISTD; 4, triprolidine HCI


Fig. 9: The chromatogram belongs to aferin syrup, 1, acetaminophen; 2, pseudoephedrine HCI; 3, sodium benzoate; 4, ISTD; 5, chlorpheniramine maleate.


Fig. 10: The chromatogram belongs to benical syrup, 1, pseudoephedrine HCI; 2, sodium benzoate; 3, ISTD; 4, chlorpheniramine maleate; 5, dextromethorphan HBr.


Fig. 11: The chromatogram belong to peditus syrup, 1, acetaminophen; 2, guaifenisin; 3, pyrilamine maleate; 4, sodium benzoate; 5, ISTD.


Fig. 12: The chromatogram belongs to kongest tablet, 1, acetaminophen; 2, ISTD; 3, chlorpheniramine maleate.


Table 5: Content of commercial cough syrup with respect to label amount claimed

Samples Compounds Labeled Amount

(mg.L-1)

 Found Amount±SD

(mg.L-1)

 Relative error

(%)
Actidem Pseudoephedrine HCI

Triprolidine HCl

Dextrrmethorphan HBr

 6000

250

2000

 5961.2±1.9

250.9±2.6

2016.1±3.9

 -0.65

+0.36

+0.81
Actifed Pseudoephedrine HCI

Triprolidine HCl

 6000

250

 6275.6±3.5

251.8±4.3

 +4.59

+0.72
Aferin Acetaminophen

Pseudoephedrine HCI

Chlorpheniramine maleate

 32000

3000

200

 32351.2±3.7

3072.8 ±1.9

207.41±1.2

 +1.10

+2.43

+3.71
Benical Pseudoephedrine HCI

Chlorpheniramine maleate

Dextromethorphan HBr

 4000

400

2000

 4021.8±1.9

398.5±4.9

2076.5±3.9

 +0.55

-0.38

+3.83
Corsal Acetaminophen

Chlorpheniramine maleate

 24000

400

 24067.8±0.9

402.6±1.7

 +0.28

+0.65
Katarin Acetaminophen

Chlorpheniramine maleate

 24000

200

 24982.4±0.3

216.4±3.4

 +4.09

+8.20
Kongest Acetaminophen

Chlorpheniramine maleate

 32000

500

 32842.3±6.1

501.55±0.9

 +2.63

+0.31
Peditus Acetaminophen

Guaifenisin

Pyrilamine maleate

 24000

10000

1250

 24412.4±6.1

10690.3±3.1

1254.4±3.01

 +1.72

+6.90

+0.35
Sudafed Pseudoephedrine HCI 6000 6003.1±2.1 +0.05

Table 6: Content of commercial cough tablet with respect to label amount claimed.

Samples Compounds Labeled Amount

(mg.L-1)

 Found Amount±SD

(mg.L-1)

 Relative error

(%)
Benical Acetaminophen

Pseudoephedrine HCI

Dextromethorphan HBr

 10000

600

400

 10010.7±1.25

600.2±1.62

397.9±1.38

 +0.11

+0.33

-0.53
Corsal Acetaminophen

Chlorpheniramine maleate

 6000

40

 5993.0±0.98

40.1±0.71

 -0.12

+0.25
Gerakon Acetaminophen

Chlorpheniramine maleate

 13000

80

 13080.1±2.21

79.8±2.76

 +0.62

-0.25
Kongest Acetaminophen

Chlorpheniramine maleate

 6000

40

 6016.6±1.45

40.67±1.92

 +0.28

+1.67
Theraflu Acetaminophen

Chlorpheniramine maleate

 13000

80

 13049.7±1.51

80.1±1.27

 +0.38

+0.18
Sudafed Pseudoephedrine HCI 1200 1205.6±1.78 +0.47

The obtained results were satisfactory for each compound. Because they show that the content of drug corresponds to the drug label. Therefore they confirm the good accuracy of the proposed method.

CONCLUSION

A basic and reliable HPLC method has been developed and validated for the determination of pseudoephdrine HCI, pheniramine maleate, acetaminophen, guaifenisin, pyrilamine maleate, chlorpheniramine maleate, triprolidine HCI, dextromethorphan HBr and diphenhydramine HCI in cough and cold pharmaceuticals. Compared to the other reported ones, the developed method offers separation of a large number of the active ingredients simultaneously. Thus large number of cough and cold pharmaceuticals could be analyzed by only one method. Forced degradation studies led to understand the chemical properties of drug molecules. Stability-indicating nature of the method was demonstrated on the experimental cough and cold syrup preparation under oxidation, acidic and alkaline, UV-light and thermal stress conditions. Although there is no acceptance criteria concerning degradation products, stability study provided to predict usage and storage conditions of the syrup.

ACKNOWLEDGMENT

I thank Dr. M. Sinan Kaynak from Department of Pharmaceutical Technology for preparation of placebo syrup. This research was supported by the İnönü University Research Council (Project no: 2010/131).

REFERENCES

  1. Caraballo I, Fernandezarevalo M, Holgado MA, Alvarezfuentes J, Rabasco AM. Simultaneous hplc determination of some drugs commonly used in cold medications-dextromethorphan, diphenhydramine, phenylephrine, phenylpropanolamine and pseudoephedrine. Drug Dev Ind Pharm 1995;21(5):605-13.
  2. Dong YM, Chen XF, Chen YL, Chen XG, Hu ZD. Separation and determination of pseudoephedrine, dextromethorphan, diphenhydramine and chlorpheniramine in cold medicines by nonaqueous capillary electrophoresis. J Pharm Biomed 2005;39(1-2):285-9.
  3. Gasco Lopez AI, IzquierdoHornillos R, Jiminez A. Development and validation of a high-performance liquid chromatography method for the determination of cold relief ingredients in chewing gum. J Chromatogr A 1997;775(1-2):179-85.
  4. Galli V, Barbas C. High-performance liquid chromatographic analysis of dextromethorphan, guaifenesin and benzoate in a cough syrup for stability testing. J Chromatogr A 2004;1048(2):207-11.
  5. Marin A, Garcia E, Garcia A, Barbas C. Validation of a HPLC quantification of acetaminophen, phenylephrine and chlorpheniramine in pharmaceutical formulations: capsules and sachets. J Pharm Biomed 2002;29(4):701-14.
  6. Shabir GA, Arain SA. Determination of paracetamol, methyl parahydroxybenzoate, ethyl parahydroxybenzoate, and propyl parahydroxybenzoate in medicinal suspension and tablets by rplc/uv-dad. J Liq Chromatogr R T 2011;34(9):719-29.
  7. Kompany-Zareh M, Mirzaei S. Spectrophotometric resolution of ternary mixtures of pseudoephedrine hydrochloride, dextromethorphan hydrobromide, and sodium benzoate in syrups using wavelength selection by net analyte signals calculated with hybrid linear analysis. Anal Chim Acta 2004;526(1):83-94.
  8. Bolser DC, Hey JA, Chapman RW. Influence of central antitussive drugs on the cough motor pattern. J Appl Physiol 1999;86(3):1017-24.
  9. Grattan TJ, Marshall AE, Higgins KS, Morice AH. The effect of ınhaled and oral dextromethorphan on citric-acid ınduced cough in man. Brit J Clin Pharm 1995;39(3):261-3.
  10. Manap RA, Wright CE, Gregory A, Rostami-Hodjegan A, Meller ST, Kelm GR, et al. The antitussive effect of dextromethorphan in relation to CYP2D6 activity. Brit J Clin Pharm 1999;48(3):382-7.
  11. Matthys H, Bleicher B, Bleicher U. Dextromethorphan and codeine-objective assessment of antitussive activity in patients with chronic cough. J Int Med Res 1983;11(2):92-100.
  12. Convention TUSP, United States Pharmacopoeia, The National Formulary. Rockville; 2002.
  13. Goodman G, The Pharmacological Basis of Therapeutics. New York: McGraw-Hill;1996.
  14. Ravisankar S, Vasudevan M, Gandhimathi M, Suresh B. Reversed-phase HPLC method for the estimation of acetaminophen, ibuprofen and chlorzoxazone in formulations. Talanta 1998;46(6):1577-81.
  15. Celma C, Allue JA, Prunonosa J, Peraire C, Obach R. Simultaneous determination of paracetamol and chlorpheniramine in human plasma by liquid chromatography-tandem mass spectrometry. J Chromatogr A 2000;870(1-2):77-86.
  16. Vasudevan M, Ravisankar S, Sathiyanarayanan A, Chandan RS. Simultaneous estimation of phenylpropanolamine HCl, guaiphenesin and diphenylpyraline HCl in syrups by LC. J Pharm Biomed 2000;24(1):25-31.
  17. Franeta JT, Agbaba D, Eric S, Pavkov S, Aleksic M, Vladimirov S. HPLC assay of acetylsalicylic acid, paracetamol, caffeine and phenobarbital in tablets. Farmaco 2002;57(9):709-13.
  18. Hood DJ, Cheung HY. A chromatographic method for rapid and simultaneous analysis of codeine phosphate, ephedrine HCl and chlorpheniramine maleate in cough-cold syrup formulation. J Pharm Biomed 2003;30(5):1595-601.
  19. Qi ML, Wang P, Zhou L, Gu JL, Fu RN. Simultaneous determination of acetaminophen, dextromethorphen hydrobromide and pseudoephedrine hydrochloride in a new drug formulation for cold treatment by HPLC. Chromatographia 2003;57(3-4):139-42.
  20. El-Gindy A, Emara S, Mostafa A. Application and validation of chemometrics-assisted spectrophotometry and liquid chromatography for the simultaneous determination of six-component pharmaceuticals. J Pharm Biomed 2006;41(2):421-30.
  21. Palabiyik IM, Onur F. The simultaneous determination of phenylephrine hydrochloride, paracetamol, chlorpheniramine maleate and dextromethorphan hydrobromide in pharmaceutical preparations. Chromatographia 2007;66:S93-S6.
  22. Manassra A, Khamis M, El-Dakiky M, Abdel-Qader Z, Al-Rimawi F. Simultaneous HPLC analysis of pseudophedrine hydrochloride, codeine phosphate, and triprolidine hydrochloride in liquid dosage forms. J Pharm Biomed 2010;51(4):991-3.
  23. Louhaichi MR, Jebali S, Loueslati MH, Adhoum N, Monser L. Simultaneous determination of pseudoephdrine, pheniramine, guaifenisin, pyrilamine, chlorpheniramine and dextromethorphan in cough and cold medicines by high performance liquid chromatography. Talanta 2009;78(3):991-7.
  24. Rowe RC, Sheskey PJ, Cook WG, Fenton ME. Handbook of Pharmaceutical Excipients. UK: Pharmaceutical Press; 2009.
  25. Mutton I, Boughtflower B, Taylor N, Brooke D. The design and use of a simple System Suitability Test Mix for generic reverse phase high performance liquid chromatography-mass spectrometry systems and the implications for automated system monitoring using global software tracking. J Chromatogr A 2011;1218(23):3711-17.
  26. Zakeri-Milani P, Barzegar-Jalali M, Tajerzadeh H, Azarmi Y, Valizadeh H. Simultaneous determination of naproxen, ketoprofen and phenol red in samples from rat intestinal permeability studies: HPLC method development and validation. J Pharm Biomed 2005;39(3-4):624-30.
  27. ICH Steering Committee,Validation of Analytical Procedures:Text and Methodology Q2(R1); 2005. p. 1-17.