Abstract

Cisplatin hydrochloride is an important chemotherapeutic drug for cancer treatment. It has a low molar absorptivity in the UV region and has no fluorescence. Therefore, a selective derivatizing reaction is required for its detection in bulk and pharmaceutical dosage form if detection by UV spectrophotometry is sought. In view of this, a simple, accurate, rapid, and cost-effective spectrophotometric method for its estimation has been developed by the complexation of the drug with ortho-phenylene diamine and monitoring the absorbance of formed green color at 706 nm. The method has been validated and successfully applied for the assay and dissolution studies of cisplatin hydrochloride tablets. The method demonstrated good linearity over the range from 0.4 to 1.4 μg/mL with a correlation coefficient of 0.9999. The accuracy of the method was 99.98%. The precision demonstrated relative standard deviation of less than 2.5%. The developed method was successfully applied for dissolution studies of sustained release tablets of cisplatin with a cumulative release of 86.7% in 12 hours. The proposed method can be applied in routine quality control in the pharmaceutical industries since it is precise, accurate, simple, and economic.

1. Introduction

Cisplatin is an important chemotherapeutic drug for cancer treatment since 1978. It is one of the complexes responsible for cell division inhibition phenomenon [1]. In order to evaluate the drug in pharmaceutical dosage forms and in clinical situations and to optimize therapeutic regimens, analytical methods capable of separating the drug from its excipients or from its individual biotransformation products and detecting these species at therapeutically relevant levels are required [2]. Several efforts have been made so far that include derivative spectrophotometry [36], detection by phosphorescence of cisplatin in urine and plasma [7], atomic absorption spectrometry [810], electroanalytical methods [11], and high-performance liquid chromatography methods [1221]. The structure of cisplatin hydrochloride is shown in Figure 1.

Cisplatin has a low molar absorptivity in the UV region and has no fluorescence. Therefore, a selective derivatizing reaction is required for the detection of drug in biological samples if the optical detection is sought. In view of this several derivatization methods have been developed but suffered from some limitations. Johnson et al. determined cisplatin in urine using derivative spectrophotometry. This method has some disadvantages as the derivatizing reaction was completed in 24 h and the reagent cannot be found easily in the market [3]. Anilanmert et al. [4] presented a method for quantification of cisplatin by complexing cisplatin with o-phenylenediamine (OPDA). The product was obtained at pH 6.2, in 30 min at 90°C, giving a maximum absorbance at 705 nm. The method was found specific for formed complex, and the maximum absorbance at 705 nm was far beyond the wavelengths of the absorption of cisplatin, o-phenylenediamine, and biomolecules in the urine. The detection limit of cisplatin in spiked urine sample was 8.40 µg/mL. The basic limitation of this method includes its higher detection limit, and the method needed to be validated. Khuhawar et al. [5] developed the spectrophotometric determination of platinum (II) from platinum-based cisplatin and carboplatin injections. In the present study platinum was treated with bis(2-hydroxynaphthaldehyde) ethylenediamine (H2HN2en) in presence of methanol at pH 8. The mixture was heated on water bath for 15 minutes at 70–75°C. The contents were allowed to cool and were transferred to separating funnel. Further the drug was extracted using chloroform, and the chloroform extract containing cisplatin was estimated at 355 nm. The major limitation of this method was the preparation of H2HN2en (prepared by condensation of 2-hydroxynaphthaldehyde with ethylenediamine in 2 : 1 molar ratio in ethanol), because this reagent is not easily available in market; the second limitation of this method is the use of multistep processes to extract out platinum followed by quantification. The extraction step may lead to inaccuracy in the quantification of drug as one has to take serious care during extraction of platinum from cisplatin. If the extraction would not be complete then it would produce error in the results; the third limitation of this method includes the need of its validation.

Edward et al. [6] also developed the method for the estimation of platinum (IV or II) by using derivatization technique with the help of o-phenylenediamine (OPDA). In this study platinum solution was treated with OPDA in presence of dimethylformamide (DMF) at pH 6.5. The solution was heated on boiling water bath for 4 min, and the developed light blue color of platinum-OPDA complex was detected at 703 nm against water as blank. This method was basically used to check the effect of pH and temperature on formation of complex and to find out the purity of platinum. Moreover, the method was needed to be validated for the desired purpose.

Most of the methods mentioned above were utilized for the clinical investigation of cisplatin, and thus the need of developing a simple, rapid, sensitive, cost-effective, and robust method is sought to quantify the drug during its regular quality control testing (e.g., assay and dissolution) and to fulfill batch release specifications.

In the present study we have used the principle of formation of complex of platinum with OPDA as used by Edward et al., to estimate the amount of cisplatin hydrochloride present in tablet dosage form. The developed method was validated as per ICH Q2 (R1) guidelines and successfully applied for assay and dissolution studies of cisplatin hydrochloride. The basic chemical reaction involved in the complex formation is shown in Figure 2.

2. Experimental

2.1. Materials

Cisplatin hydrochloride was obtained as a gift sample from Astron Research Limited, Gujarat, India. o-Phenylenediamine and potassium dihydrogen orthophosphate were purchased from CDH Laboratories, Mumbai, India. Dimethylformamide (DMF) was purchased from Loba Chemie Pvt. Ltd., Mumbai, India. Sodium hydroxide flakes were purchased from Loba Chemie, Mumbai, India. All other chemicals and reagents used were of analytical grade. Triple distilled water was used throughout the study. Analysis was done using double beam UV-Visible spectrophotometer (Shimadzu 1800, Japan).

2.2. Methods
2.2.1. Spectrophotometric Measurements

The spectra of different concentrations of reference solutions of Cisplatin hydrochloride were recorded in 1 cm glass cells at a fast scan speed. The spectrophotometric measurements were recorded by using mixture of 1.4 mg/mL of OPDA solution, phosphate buffer pH 6.8, and DMF (1 : 2 : 7) as a blank solution as shown in Figure 3.

2.2.2. Analytical Method Development

(1) Development of Colour and Preparation of Calibration Curve. Ten milligrams of cisplatin hydrochloride working standard was weighed accurately and transferred to 100 mL standard volumetric flask, and the volume was adjusted to 100 mL using phosphate buffer pH 6.8 in order to get a concentration of 100 μg/mL. 10 mL of sample aliquot was withdrawn from this stock solution and was diluted to obtain the known standard concentration of 10 μg/mL. From this, 0.4, 0.6, 0.8, 1.0, 1.2, and 1.4 mL of aliquots were withdrawn in 10 mL standard volumetric flask, and then 1 mL of 1.4 mg/mL of OPDA solution and 2 mL of phosphate buffer pH 6.8 were added and heated at 100°C for 10 min in order to get light green colour solution. The prepared coloured solutions were cooled to room temperature, and finally the volume was made up to 10 mL using DMF and measured at 706 nm using a UV-Visible spectrophotometer.

(2) Sample Solutions. Twenty tablets of cisplatin hydrochloride were used. The tablets were weighed and triturated, and the contents were thoroughly mixed. The mass equivalent to 150 mg of cisplatin was weighed into a 250 mL volumetric flask, and phosphate buffer pH 6.8 was added to make up the volume. Appropriate dilutions were made using 1 mL of 1.4 mg/mL of OPDA solution and 2 mL of phosphate buffer pH 6.8 and heated at 100°C for 10 min in order to get light green colour solution. The prepared coloured solutions were cooled to room temperature, and finally the volume was made up to 10 mL using DMF.

(3) Stability of Cisplatin in Solution. The stability of cisplatin hydrochloride standard stock solution in a mixture of 1.4 mg/mL of OPDA solution, phosphate buffer pH 6.8, and DMF at a concentration of 0.8 μg/mL was investigated at different time intervals using the experimental conditions.

2.2.3. Validation of the Developed Method

(1) Linearity and Range. Linearity of the curve in the concentration range had been assessed by calibration curve using solutions of 0.4, 0.6, 0.8, 1.0, 1.2, and 1.4 μg/mL, respectively. Measurements were taken on samples prepared on 3 consecutive days (). The values are reported as the mean ± confidence interval of the calibration curves. The data was analyzed at a wavelength of 706 nm. Evaluation parameters such as the correlation coefficient were calculated and are presented.

(2) Specificity Studies. Specificity was evaluated by an analysis of the visible spectrum of placebo solutions, cisplatin hydrochloride working standard solution, and cisplatin hydrochloride sample solution at concentration of 0.8 μg/mL. The placebo solution was prepared with the same composition as the formulation without the addition of cisplatin hydrochloride and treated in the same manner as the commercial sample solution and the reference solution. The solution was filtered through 0.45 micron membrane filter and then subjected for UV analysis. The results of specificity studies are shown in Figure 4.

(3) Accuracy. The accuracy of the method was determined by measuring the reference standard recovery in triplicate at three levels, 50%, 100%, and 150% of the method concentration (0.8 µg/mL). A standard stock solution 100 µg/mL of cisplatin was prepared as described in Section 2.2.2. In volumetric flasks of 100 mL, aliquots of 0.4, 0.8, and 1.2 mL of this solution (which would yield concentrations of 0.4, 0.8, and 1.2 µg/mL, resp.) were combined with 0.134 mL of the 600 µg/mL sample solution from Section 2.2.2 (this would yield a concentration of 0.8 µg/mL). Dilutions were made using 1 mL of 1.4 mg/mL of OPDA solution and 2 mL of phosphate buffer pH 6.8 and heated at 100°C for 10 min in order to get light green colour solution. The prepared colored solutions were cooled to room temperature, and finally the volume was made up to 10 mL using DMF. Thus the final concentrations were 1.2, 1.6 and 2.0 µg/mL, which correspond to 50, 100 and 150% of the target concentration, respectively. The mean recoveries of cisplatin (150 mg), expressed in terms of the percentage recovery and relative standard deviation (%R.S.D.), were determined.

(4) Precision. Precision was evaluated with respect to both repeatability and intermediate precision. Repeatability was tested by seven determinations at three levels, 50%, 100%, and 150% of the method concentration (0.8 μg/mL) on the same day and under the same experimental conditions. Intermediate precision was evaluated by performing the analysis on three different days (interday) on the same levels as mentioned above and by the three analysts performing the analysis in the same laboratory and under the same experimental conditions (between analyst). Seven replicates at concentrations of 0.4, 0.8, and 1.2 μg/mL were prepared and assayed at 706 nm. The percentage of relative standard deviation (R.S.D.) of the analytical responses was calculated.

(5) Robustness. The robustness of analytical method is measure of its ability to remain unaffected by small changes. In the present study robustness has been calculated by varying the pH and taking the absorbance at pH 6.6, pH 6.8 and pH 7.0 of the sample solution (cisplatin hydrochloride 150 mg). Moreover, the robustness of the method was determined by analyzing a change of 2 nm in the wavelength of analysis. Seven replicates of the working standard solution and sample solution were prepared at the same concentration (0.8 μg/mL), and the assays were carried out at 704, 706, and 708 nm. The percentage relative standard deviation (R.S.D.) of the quantitation of cisplatin hydrochloride in the tablets was calculated.

(6) Limit of Detection (LOD) and Limit of Quantification (LOQ). Estimation of LOD and LOQ was determined by standard deviation of response (σ) and slope of calibration curve (). Standard deviation of   intercepts of regression line was used as standard deviation. Equations (1) and (2) for LOD and LOQ, respectively, are as follows:

2.2.4. Application of Validated Method to Assay and Dissolution Studies of Cisplatin Hydrochloride Tablets

(1)  Assay of Cisplatin Hydrochloride Tablets. The validated UV-spectrometric method was applied to cisplatin hydrochloride quantitation of the (cisplatin hydrochloride tablets 150 mg). The results were obtained by comparing the sample spectrophotometric measurements () with those obtained from the cisplatin hydrochloride standard solutions () at the same concentration levels.

(2) Dissolution Studies. The dissolution study of cisplatin hydrochloride tablets (150 mg) was carried out in 900 mL phosphate buffer pH 6.8 at 50 rpm. From the dissolution medium, 5 mL samples were withdrawn at 0.25, 0.5, 1, 2, 3, 4, 6, 9, and 12 h, respectively. From this, 1 mL of solution was pipetted out, and diluted to 10 mL by using phosphate buffer pH 6.8. Again from the diluted solution, 1 mL solution was pipetted out and dilutions were made by using 1 mL of 1.4 mg/mL of OPDA solution and 2 mL of phosphate buffer pH 6.8 and heated at 100°C for 10 min in order to get light green colour solution. The prepared coloured solutions were cooled to room temperature, and finally the volume was made up to 10 mL using DMF which were measured at 706 nm using a UV-Visible spectrophotometer. The study was conducted for 6 tablets, and the mean % cumulative drug release was recorded ().

3. Results and Discussions

3.1. Method Development

The reported methods for the determination of cisplatin were complex and time consuming. Moreover, some methods were developed on sophisticated instruments like HPLC which have higher costs. Precolumn derivatization of cisplatin hydrochloride (as it lacks chromophore) followed by HPLC analysis makes the process tedious and expensive. In this paper, phosphate buffer pH 6.8, OPDA, and DMF were chosen to obtain an inexpensive, simple, and environment friendly colorimetric method for the quantification of cisplatin hydrochloride in tablets.

3.2. Stability of Cisplatin in Solution

The results from the stability study indicated that the cisplatin hydrochloride stock standard solution was stable at room temperature for at least one week (Table 1).

3.3. Method Validation

After the method development, the analytical method was validated according to ICH recommendations.

3.3.1. Linearity and Range

The analytical curves, obtained on three consecutive days () by plotting the mean of absorbance at 706 nm against the concentration, were found to be linear in the 0.4 to 1.4 μg/mL range and yielded a correlation coefficient () of 0.9994 shown in Table 2 and Figure 5.

3.3.2. Selectivity

The spectra analysis showed that the formulation excipients of the pharmaceutical tablet product containing cisplatin hydrochloride tablets 150 mg did not interfere with the developed colorimetric method as shown in Figure 4. The spectrum showed that the placebo did not have absorbance in the wavelength used in this method.

3.3.3. Accuracy

The accuracy of the proposed method was assessed by determining the average recoveries of samples using the standard addition method. As shown in Table 3, the mean percentage recovery of cisplatin hydrochloride tablets (150 mg) was 99.59%, and the % relative standard deviation (%R.S.D.) was 0.76%. The results were in accordance with fixed limits from 98.0% to 102.0%, indicating the suitability of the developed method in quantifying the concentration of cisplatin hydrochloride in tablets. The accuracy value of the current method was found to beexcellent should be written as be excellent.

3.3.4. Precision

The precision, evaluated as the repeatability of the analytical method, was studied by calculating the % relative standard deviation for the seven determinations of the 0.4, 0.8, and 1.2 μg/mL working standard solution performed on the same day and under the same experimental conditions. The obtained %R.S.D. value was less than 2.5%. The intermediate precision was assessed by analyzing a sample of the pharmaceutical formulation on 3 different days (interday precision) and by analyzing the samples with three analysts (between-analysts precision). The %R.S.D. values were less than 2.5% confirming that the method is sufficiently precise (Table 4).

3.3.5. Robustness

The robustness was found reliable, as determined by %R.S.D. (<2%). It was observed that the constancy of the absorbance with deliberative changes in the experimental parameter of wavelength resulted in a %R.S.D. of 0.81 and change in pH resulted in a %R.S.D. of 0.72 (Table 5). The minor changes that occurred during the analysis did not affect the absorbance intensity of the samples.

3.3.6. Limits of Detection and Quantification

LOD and LOQ values were found to be 0.038 ± 0.056 and 0.116 ± 0.058 μg/mL, respectively, for cisplatin hydrochloride tablets (150 mg). These results demonstrated that the analyses were being performed in a region above the quantification limit value.

3.3.7. Assay of Cisplatin Hydrochloride Tablets

The validated method was applied to the determination of cisplatin hydrochloride in tablets. Three samples of cisplatin hydrochloride tablets (150 mg) were analyzed. The results, expressed as the percentage drug as related to the content label claim, are shown in Table 6. The results showed that the percentage drug is in accordance with the Indian, British, and United States Pharmacopoeias, which permit cisplatin hydrochloride in tablets to be in a range from 92.5 to 110.0% of the content label claim.

3.3.8. Dissolution Studies

An analytical method should be developed in such a way that it should be able to evaluate all the parameters quantitatively during the early product development stage till the final product release. Dissolution studies play a major role in order to provide drug release testing during early preformulation studies as well as in vitro-in vivo correlation of the compound during the bioavailability studies and clinical trials. Therefore dissolution studies were conducted in order to check the feasibility of this developed and validated method for quantification of dissolution samples. The mean % cumulative drug release was found to be 86.74% after 12 h. The dissolution profile of cisplatin hydrochloride tablets (150 mg) is shown in Figure 6. This showed that the developed method can be successfully applied to dissolution studies.

UV, UV-VIS, and derivative spectrophotometry are broadly used techniques to quantify antibiotics and other drugs because they are cost effective and simple and do not require time-consuming sample preparation compared to other techniques. Moreover, UV-Visible spectrophotometry produces very low amount of residues and solvents, which is an important ecological aspect as per regulatory point of view and currently discussed in routine laboratory analysis. Because of these reasons and the careful validation of this method, this technique can be recommended for the routine laboratory analysis of the cisplatin hydrochloride in tablets.

4. Conclusion

The validated analytical method for quantitative determination of cisplatin hydrochloride in tablets has the advantages of simplicity, speed, low-cost conditions, and a lack of polluting reagents. All validation parameters were found to be highly satisfactory, including linearity, accuracy, precision, selectivity, robustness, and adequate detection and quantitation limits. The validated method could be a good alternative for routine quality control of cisplatin hydrochloride by the pharmaceutical industries and quality control laboratories.

Acknowledgments

The authors are grateful to Mr. Ashok Mittal, Chancellor, Lovely Professional University, India for providing facilities to carry out the aforementioned research. Theye also owe their thanks to Astron Research Limited, Gujarat, India, for providing the gift samples of cisplatin hydrochloride.