Received- July 16, 2009; Accepted- September 29, 2009
 International Journal of Biomedical Science 5(4), 421-427, Dec 15, 2009
Original Article


© 2005 Master Publishing Group

A Sensitive Spectrophotometric Method for the Determination of Pregabalin in Bulk, Pharmaceutical Formulations and in Human Urine Samples

Rajinder Singh Gujral, Sk Manirul Haque, Prem Shanker

Vardhman Chemtech Ltd, Nimbua, Dera Bassi, Mohali (Punjab) India

Corresponding Author: Rajinder Singh Gujral, Director, Vardhman Chemtech Ltd, Nimbua, Dera Bassi, Mohali, Punjab, India. E-mail: gujral@vardhmanchemtech.com.

Running title: Determination of Pregabalin by Spectrophotometry


  ABSTRACT
INTRODUCTION
EXPERIMENTAL
METHODS
RESULTS AND DISCUSION
CONCLUSIONS
REFERENCES


 ABSTRACT

A simple and sensitive spectrophotometric method was developed and validated for the determination of pregabalin in bulk, pharmaceutical formulations and in human urine samples. The method was based on the reaction of drug with the mixture of potassium iodate and potassium iodide. The method was linear in the range of 0.5-3.5 µg/ml. There is no official method for the determination of pregabalin. The absorbance was measured at 353 nm. The method was validated with respect to accuracy, precision, specificity, ruggedness, robustness, limit of detection and limit of quantitation. This method was used successfully for the quality assessment of five pregabalin drug products and in human urine samples with good precision and accuracy.

KEY WORDS:    pregabalin; validation; bulk drug, pharmaceutical formulations; human urine samples

 INTRODUCTION

   Pregabalin [S-[+]-3-isobutyl GABA or (S)-3-(amino methyl)-5-methylhexanoic acid, Lyrica] (Fig. 1) is an anticonvulsant and analgesic medication that is both structurally and pharmacologically related to gabapentin (Neurotonin; Pfizer Inc; New York, NY). It was recently approved for adjunctive treatment of partial seizures in adults (1-4) in both the United States and Europe and for the treatment of neuropathic pain from postherpetic neuralgia and diabetic neuropathy. The compound was originally synthesized with the hope of modulating brain GABA receptors or GABA synthetic enzymes. These compounds are inactive at GABAA and GABAB receptors. The mechanism of action of Pregabalin has been characterized only partially, and in particular, the cellular and molecular details of its action to reduce neurotransmitter release are incompletely known.

   Pregabalin undergoes minimal metabolism in human with unchanged parent representing the majority (≥90 %) of drug-derived material (5). This contrasts with gabapentin, which is absorbed via a capacity limited L-amino acid transport system from the proximal small bowel into the blood stream (6, 7).

   The therapeutic importance of Pregabalin was behind the development of numerous methods for its determination. The methods adapted to the analysis of PGB include high–performance liquid chromatography (HPLC) (8), liquid chromatography-mass spectrophotometry (LC-MS) (9, 10) and spectrofluorimetry (11). The determination in biological fluids normally requires the use of trace analysis techniques such as HPLC, LC, capillary electrophoresis (CE), cyclic voltametry, LC-MS, gas chromatography – mass spectrophotometry (GC-MS), inductively coupled plasma – mass spectrophotometry. These methods require long and tedious pretreatment of the samples and laborious clean up procedures prior to analysis. An official monograph of PGB does not exist in any pharmacopoeia and determination of PGB in bulk and pharmaceutical formulations has not been yet described. Therefore, it is very imperative to develop a simple and suitable analytical method for the determination of PGB in bulk and pharmaceutical formulations. UV-Visible spectrophotometry is the technique of choice in research laboratories, hospitals and pharmaceutical industries due to its low cost and inherent simplicity.

   This paper reports a simple, sensitive and accurate spectrophotometric method for the determination of PGB. The method was based on the reaction of drug with the mixture of potassium iodide and potassium iodate and absorbance was measured at 353 nm. The proposed method was extended to the determination of PGB in bulk, pharmaceutical formulations and in human urine samples.

 EXPERIMENTAL

   Apparatus

   Spectral runs were made on UV 3000+ UV/VIS spectrophotometer (LABINDIA®, Mumbai, India) with 1 cm matched glass cell.

   Materials and Reagents

   Standard PGB Solution

   A stock solution of PGB (50 µg/ml) was prepared by dissolving 5 mg PGB in 100 ml volumetric flasks with double distilled water. The stock solution (50 µg/ml) was used to prepare the working solutions by suitable dilutions with distilled water. The solutions were stable at least 10 days in room temperature.

 METHODS

   Procedure for the determination of PGB

   Aliquots of stock solution (50 µg/ml) were pipetted into a series of 10 ml volumetric. To each flask, 1.0 ml 4 × 10-2 M KI and 2.5 ml 5 × 10-3 M KIO3 were added and diluted to volume with distilled water. The reaction was allowed to proceed at room temperature. The calibration curve was constructed by plotting absorbance against the initial concentration of PGB. The linearity range or Beer’s range follows in the range between 0.5 to 3.5 μg/ml (Fig. 2). The content of PGB was calculated either from the calibration curve or corresponding regression equation and found that the absorbance is stable for at least ten days at room temperature.

   Procedure for determination of PGB in pharmaceutical formulations

   One capsule (claiming 75 mg of Pregabalin) was accurately weighed and finely powdered. A quantity of the powder equivalent to 5 mg of PGB was extracted by shaking with 20 ml of distilled water, followed by another two extractions each with 10 ml distilled water. After passing through a 0.45 μm Millipore filter, the solution was diluted with distilled water to obtain a concentration of about 50 µg/ml. It was further diluted according to the need and then analyzed following the proposed procedures. The nominal content of the capsule was calculated either from the previously plotted calibration graphs or using regression equation.

   Procedure for determination of PGB in human urine samples

   Aliquot volumes of human urine samples were transferred into small separating funnel. 10 ml of carbonate buffer pH-9.4 was added and solution was mixed well. The solution was then extracted with 3 × 10 ml diethyl ether. The ether extract was collected and evaporated. The residue was dissolved in 10 ml distilled water and above general procedure was then followed. The amount of PGB was obtained from the calibration graphs or corresponding regression equation.

 RESULTS AND DISCUSION

   Reaction with a mixture of iodide and iodate

   It has been reported in the literature (12) that iodine is formed as a result of the interaction of a mixture of iodide and iodate with inorganic or organic acid in accordance with the equation:

   5 I- + IO3- + 6 H+ → 3 H2O + 3 I2

   In aqueous medium, the iodide ions react with the liberated iodine to yield triiodide ion (I2 + I- → I3-) which detected in UV detector at 353 nm. We thought that this reaction would be helpful for developing a spectrophotometric method for determination of PGB as it contains - COOH group in its moiety. Keeping this in mind, a mixture of potassium iodide and iodate was allowed to react with PGB which yielded iodine. Then the liberated iodine reacted with the excess of iodide ion resulting in the formation of triiodide ion (Fig. 3).

   Optimization of reaction conditions

   The different parameters affecting the development process were extensively studied to determine the optimum conditions for the assay procedures. The optimum values of the variables were maintained throughout the determination process.

   Effect of the concentration of potassium iodate: The effect of the volume of 5 × 10-3 M potassium iodate on the absorbance of the product was studied in the range of 0.2-2.8 ml. The absorbance increases with the increase in the volume of potassium iodate and became constant at 2.2 ml. Further addition of KIO3 does not change in the absorbance and therefore, 2.5 ml of 5 × 10-3 M KIO3 was chosen as an optimum value (Fig. 4).

   Effect of the concentration of potassium iodide:The effect of the volume 4 × 10-2 M potassium iodide on the absorbance of the product was studied in the range of 0.1-1.2 ml, keeping the constant concentrations of PGB (50 µg/ml) and KIO3 (12.5 × 10-3 M). The maximum absorbance was obtained with 0.8 ml; further addition caused no change on the absorbance. Thus, 1.0 ml of 4 × 10-2 M potassium iodide (Fig. 5) was used throughout the experiment.

   Method Validation

   The method was validated for selectivity, linearity, precision, accuracy, recovery and stability according to the principles of the Food and Drug Administration (FDA) industry guidance (13). The specificity and selectivity of the proposed method was evaluated by estimating the amount of PGB in the presence of common excipients lactose monohydrate, corn, starch, talc and methyl cobalamin.

   The linearity of the proposed method was constructed for Pregabalin reference standard solution by plotting concentration of the compound versus the absorbance. The linearity was evaluated by linear regression analysis, which was calculated by the least square regression method. The parameters LOD and LOQ were determined on the basis of response and slope of the regression equation. The accuracy and precision of the method was evaluated within the linear range based on the analysis of PGB reference standard samples and pharmaceutical formulations at 1.0, 2.0 and 3.0 µg/ml. Five independent analysis were performed at each concentrations level within one day (intraday precision) as well as for five consecutive days (interday precision). The accuracy was ascertained by recovery studies using the standard addition method. The proposed method was used for estimation of PGB from capsules after spiking with 50, 150 and 250 % additional pure drug. The amount of PGB was determined from the regression equation.

   The absorbance-concentration plot for the proposed method was found to be rectilinear over the range of 0.5-3.5 µg/ml.  Linear regression analysis of calibration data gave the regression equation cited in Table 1 with correlation coefficients close to unity. Statistical analysis of regression lines were made regarding the standard deviation of residuals (Sx/y), standard deviation of slopes (Sb) and standard deviation of intercepts (Sa) and the values are summarized in Table 1.

   The within day precision assays were carried out through replicate analysis (n=5) of PGB corresponding to 1.0, 2.0 and 3.0 µg/ml. The interday precision was evaluated through replicate analysis of the pure drug samples for five consecutive days at the same concentration levels as used in within day precision. The results of these assays are reported in Table 2. As can be seen from Table 2 that the recovery and RSD values for within day precision were always lower than 100.10% and 0.799%; recovery and RSD values for interday precision were lower than 100.07% and 1.001%. The precision results are satisfactory. The intraday and interday precision assays were also carried for PGB in pharmaceutical formulations. The results are summarized in Table 3. As can be seen from Table 3 that the recovery and RSD values were in the ranges 99.85 to 100.07%; 0.133 to 1.20% and 99.90 to 100.10%; 0.167 to 1.001% respectively for intraday and interday precision.

   The proposed method was used for estimating of PGB from capsules after spiking with 50, 150 and 250 % of additional pure drug. The results are reported in Table 4. As can be seen from Table 4 that the recovery and RSD values were in the ranges 99.867 to 100.067 % and 0.200 to 0.800 %. The selectivity of the proposed method was ascertained by analyzing standard PGB in the presence capsule such as lactose monohydrate, corn, starch, talc and methyl cobalamin. It was observed that the excipients did not interfere with the proposed method.

   The proposed method was further extended to the in vitro determination of PGB in spiked human urine samples. In neuropathic patients, PGB is orally given in doses of 150 to 600 mg per day, with an associated mean of around 123 µg.hr/ml. Pregabalin undergoes minimal metabolism in human with unchanged parent representing ≥ 90% of drug derived in urine. This concentration fell well in within working range of proposed method. The calibration graphs were constructed by plotting absorbance versus increasing concentrations of PGB in spiked human urine samples over the concentration range 0.5-3.5 µg/ml. The results (Table 5) are satisfactorily accurate and precise. The performance of the proposed method was studied with other existing method (14). In case of proposed method and reported method, the reported method has higher LOD and LOQ value than the proposed method and summarized in Table 6.


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Figure 1.  Structure of Pregabalin.
 

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Figure 2.  Linear Regression equation of the proposed method.
 

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Figure 3. This is reaction mechanism of formation of TriIodide ion.
 

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Figure 4. Effect of the volume of KIO3 (5.0 × 10-3 M); keeping constant 0.5 ml of 50 µg/ml PGB and KI (3.2 × 10-2 M).
 

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Figure 5. Effect of the volume of KI (4.0 × 10-2 M); keeping constant 0.5 ml of 50 µg/ml PGB and KIO3 (12.5 × 10-3 M).

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Table 1. Summary of optical and regression characteristics of the proposed method


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Table 2. Summary of accuracy and precision results of the proposed method in pure form.


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Table 3. Summary of accuracy and precision results of the proposed method in pharmaceutical formulations


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Table 4. Summary of data for the determination of pregabalin in pharmaceutical preparations by standard addition method


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Table 5. Application of the proposed spectrophotometric method to the determination of pregabalin in human urine samples


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Table 6. Comparable table for the proposed method and reported method (14)

 CONCLUSIONS

   The proposed method does not require any laborious clean up procedure before measurement. In addition, the method has wider linear dynamic range with good accuracy and precision. The method shows no interference from the common excipients and additives. This may help in analyzing affectivity of this drug in human beings during treatment. Therefore, it is concluded that the proposed method is simple, sensitive and rapid for the determination of PGB in bulk, pharmaceutical formulations and in human urine samples.  

 REFERENCES

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