Abstract

Titrimetric and spectrophotometric assay of ganciclovir (GNC) is described using cerium(IV) sulphate as the oxidimetric reagent. The methods are based on the oxidation of GNC with a measured excess of cerium(IV) sulphate in acid medium followed by determination of the unreacted oxidant by two different reaction schemes. In titrimetry, the unreacted oxidant was determined by back titration with ferrous ammonium sulphate (FAS) in sulphuric acid medium, and spectrophotometry involves the reaction of residual cerium(IV) with p-DMAB to form brownish-coloured p-dimethylamino quinoneimine whose absorbance was measured at 460 nm. In both methods, the amount of cerium(IV) sulphate reacted corresponds to GNC concentration. Titrimetry is applicable over 3–10 mg range where as, in spcetrophotometry, the calibration graph is linear over the range of 2–10 μg mL−1 and the calculated molar absorptivity value is 1.960×104 L mol−1 cm−1. The validity of the proposed methods was tested by analyzing pure and dosage forms containing GNC. Statistical treatment of the results reflects that the proposed procedures are precise, accurate, and easily applicable for the determination of GNC pure form and in pharmaceutical formulations.

1. Introduction

Ganciclovir (GNC) chemically known as 2-amino-9-{[(1,3-dihydroxypropan-2-l)oxy]methyl}-6,9-dihydro-3H-purin-6-one (Figure 1) is a nucleoside analogue widely used in the treatment of cytomegalovirus infections.

It has been proved effective against cytomegalovirus in immunocompromised patients, mainly in those with the acquired immunodeficiency syndrome (AIDS), congenital immunodeficiency, or in individuals following organ transplantation [1, 2]. Various techniques have been developed for the determination of GNC in pharmaceuticals. It is official in the United States Pharmacopoeia [3].

The most extensively used technique for the quantitation of ganciclovir is HPLC, but most of the procedures using this technique are devoted to body fluids like plasma [818], tissues [19], serum [20], and blood samples [21]. HPLC has also been applied for the determination of GNC in eye drops [22]. GNC in bulk drug and in its formulations has been assayed by UV-spectrometry by measuring the absorbance of drug in 0.1 M HCl and 0.1 M NaOH at 253 and 266 nm, respectively. The methods are reported to be moderately sensitive with molar absorptivity values of ~2.0×103. There are only three reports on the use of visible spectrophotometry for the assay of GNC in pharmaceuticals. Schelling et al. [4] have devised an enzyme kinetic method which involves the use of multiple reagents and scrupulously controlled experimental variables. The procedure also requires expensive radiolabelled substrates. Recently, Gouda [5] has reported the application of five σ-and π-acceptors for the spectrophotometric determination of GNC in its formulations via charge-transfer complexation reaction. The methods have been found applicable over 5–225 μg mL−1 ranges with limits detection (LOD) values in the range of 0.36–2.45 μg mL−1. In a very recent report, [6] Sarsambi et al. have described two procedures based on Schiff base formation using p-dimethylamino cinnamaldehyde and oxidative coupling reaction involving the use of iron(III) and MBTH, but the methods are poorly sensitive and require heating at 40°C, with linear dynamic range of 10–50 μg mL−1 and 50–250 μg mL−1, respectively. The methods also employ expensive reagents. A flow injection chemiluminescence method has also been described by Wang et al. [7]. Though the method appears to be sensitive with an LOD of 2.35 μg mL−1, it requires a complicated and expensive flow-injection assembly as shown in Table 1.

No titrimetric method has ever been reported for GNC despite its simplicity and versatility. In this paper, titrimetric and spectrophotometric determination of GNC is described. The methods are based on the oxidation of drug with a measured excess of Ce(IV) sulphate followed by the determination of residual oxidant either by titration with iron(II) in titrimetry or by spectophotometry involving the use of Ce(IV) and p-DMAB. The developed methods were optimized and validated as per the guidelines of the International Conference on Harmonization [23]. The methods are important alternatives to other analytical methods with clear advantages in terms of simplicity, cost effectiveness, speed, and sensitivity.

2. Materials and Methods

2.1. Instrument

Absorbance measurements were made on a Systronics model 106 digital spectrophotometer (Ahmedabad, India) provided with 1 cm matched quartz cells.

2.2. Material and Reagents

All chemicals and reagents used were of analytical or pharmaceutical grade and distilled water was used to prepare the solutions.

Sulphuric Acid (0.1 M; 0.5 M; 2 M; 5 M)
It was prepared by appropriate dilution of the conc. H2SO4 (SD Fine Chem, Mumbai, India, sp. gr. 1.84) with water.

Perchloric Acid (HClO4; 4 M)
It was prepared by diluting concentrated acid (Merck, Mumbai, India, assay 70%) appropriately with water to get 4 M for spectrophotometric method.

Cerium(IV) Sulphate Solution (0.02 M and 300 μg mL−1)
A stock standard solution equivalent to 0.02 M cerium(IV) sulphate was prepared by dissolving 4.04 g of the chemical (Loba Chemie, Mumbai, India, assay 99.9%) in 14 mL of conc. H2SO4 and diluting to 500 mL with water in a 500 mL standard flask, mixed well, filtered using glass wool, standardized [24] and used in titrimetric work. The stock solution was then diluted appropriately with 4 M HClO4 to obtain a working concentration of 300 μg mL−1 in cerium(IV) sulphate for spectrophotometric method.

Ferrous Ammonium Sulphate Solution (0.02 M)
A stock solution of FAS (0.02 M) was prepared by dissolving 3.92 g of the chemical (Loba Chemie, Mumbai, India, assay 99–101%) in water containing 5 mL of 0.5 M H2SO4 and diluted to volume in a 500 mL calibrated flask with water and used in titrimetric assay.

Ferroin Indicator Solution
It was prepared by dissolving 1.485 g of 1,10-phenanthroline monohydrate and 0.695 g of FeSO4·7H2O in water and diluted to 100 mL [25].

Dimethylaminobenzaldehyde (p-DMAB; 0.5%)
An accurately weighed 1.25 g of p-DMAB (Merck, Mumbai, India) was transferred to a 250 mL volumetric flask, dissolved in 4 M HClO4 and the volume was made up to the mark with the same solvent.

Standard GNC Solution (1 mg mL−1 and 20 μg mL−1)
A stock standard solution containing 1 mg mL−1 GNC was prepared by dissolving 100 mg of pure GNC in 0.1 M H2SO4 the volume was brought to 100 mL with water in a volumetric flask and used for titrimetric assay.
A 100 μg mL−1 GNC standard solution was also prepared by dissolving an accurately weighed 10 mg of GNC in 4 M HClO4 and diluting to the mark with the same solvent in a 100 mL calibrated flask, and this was diluted with the same solvent to get a working concentration of 20 μg mL−1 GNC and used spectrophotometric method.
Two brands of tablets containing GNC, Ganguard-500 (Ranbaxy, Superspeciality Ltd., Ahamadabad, India) and Nataclovir-250 (Natco Pharma Ltd., Hyderabad, and India) used in the investigation were purchased from local commercial sources.

2.3. Methods

Titrimetry
A 10 mL aliquot of standard drug solution in 0.1 M H2SO4 containing 1–10 mg of GNC was measured accurately and taken in a 100 mL titration flask; 5 mL of 0.1 M H2SO4 and 2 mL of 2 M H2SO4 were added to the flask. By means of a pipette, 10 mL of 0.02 M Ce(IV)SO4 was added, content-mixed and the flask kept aside for 15 min. Then, the unreacted cerium(IV) solution was titrated against 0.02 M FAS using ferroin indicator to a first appearance of orange red color. A blank titration was performed with 10 mL 0.1 M H2SO4 in place of GNC solution.
The amount of GNC in the aliquot was computed from the formula: Amount(mg)=𝑉𝑀𝑤𝑆𝑛,(1) where 𝑉 is mL of cerium(IV) sulphate reacted, 𝑀𝑤 is relative molecular mass of drug, 𝑆 is strength of cerium(IV) sulphate, moles L−1, and 𝑛 is number of moles of cerium(IV) sulphate reacting with per mole of GNC.

Spectrophotometry
Varying aliquots (0.0, 1.0, 2.0, 3.0, 4.0, and 5.0 mL) of 20 μg mL−1 GNC solution were transferred into a series of 10 mL calibrated flasks by means of a microburette and the total volume was adjusted to 5 mL by adding requisite volume of 4 M HClO4. To each flask 1 mL of 300 μg mL−1 Cerium(IV) sulphate was added from a microburette. The content was mixed well and the flasks were let stand for 10 min with occasional shaking. Then, was added 1 mL of 0.5% p-DMAB to each flask, again the flasks were let stand for 5 min. The volume was diluted to the mark with 4 M HClO4, mixed well and the absorbance of each solution was measured at 460 nm against water.
A calibration graph was prepared by plotting the measured absorbance versus concentration of GNC, and the concentration of the unknown was red from the calibration graph or deduced from the regression equation derived using the Beer’s law data.

Procedure for Tablets
Twenty tablets were weighed accurately and finely powdered. A quantity of the powdered tablet containing 100 mg of GNC was weighed accurately and transferred into a 100 mL calibrated flask, 60 mL of 0.1 M H2SO4 was added, and the content was shaken thoroughly for 15–20 min to extract the drug into the liquid phase; the volume was finally diluted to the mark with 0.1 M H2SO4, mixed well and filtered using a Whatman no. 42 filter paper. First 10 mL portion of the filtrate was discarded, and a convenient aliquot of the subsequent portion of filtrate was subjected to analysis by titrimetry.
The tablet extract containing GNC at a concentration of 1 mg mL−1 was then diluted stepwise with 4 M HClO4 to obtain a working concentration of 20 μg mL−1 in GNC and a convenient aliquot was then subjected to analysis by spectrophotometer procedure described earlier.

Placebo Blank Analysis
A placebo blank of the composition: talc (20 mg), starch (10 mg), acacia (15 mg), methyl cellulose (10 mg), sodium citrate (10 mg), magnesium stearate (15 mg), and sodium alginate (10 mg) was made and its solution was prepared as described under “procedure for tablets,” and then subjected to analysis.

Procedure for the Determination of GNC in Synthetic Mixtures
To the placebo blank of the composition described above, 100 mg of pure GNC was added and homogenized, transferred to a 100 mL standard flask, and solution-prepared as described under “procedure for tablets.” The resulting solution was assayed (𝑛=5) by titrimetry according to the same procedure described above.
The synthetic mixture solution (1 mg mL−1 in GNC) was then diluted stepwise with 4 M HClO4 to obtain a working concentration of 20 μg mL−1 in GNC for spectrophotometric method. A convenient aliquot was then subjected to analysis by spectrophotometric procedure described above. The analysis was done to study the interferences from excipients such as talc, starch, acacia, anhydrous lactose, sodium alginate, magnesium stearate, and methyl cellulose.

3. Results and Discussions

The proposed methods are indirect and are based on the determination of unreacted cerium(IV), after the reaction between GNC and the oxidant is ensured to be complete, and rely on two different well-known reactions which are shown below GNC+Ce(IV)(knownacess)H+OxidationproductofGNC+UnreactedCe(IV)UnreactedTitratedwithstandardFASusingferroinindicator(Titrimetry)Unreacted+p-DMABinHClO4Orangecolouredproductmeasuredmediumat460nm(Spectrophotometry).(2)

The titrimetric method involves oxidation of GNC by a known excess of cerium(IV) sulphate in H2SO4 medium and the unreacted oxidant was determined by back titration with FAS. The reaction between GNC and cerium(IV) was found to occur in 1 : 1 (drug : oxidant) stoichiometric ratio and all the calculations are based on this stoichiometric ratio. Using 0.02 M cerium(IV), 3–10 mg of GNC was conveniently determined.

Redox reactions always preferred highly acidic conditions. The oxidation reactions of some compounds are very rapid when perchloric acid (HClO4) medium is maintained [2629]. This is attributed to the highest oxidation potential of cerium(IV) in HClO4 (𝐸𝑜 = 1.75 V) as compared to that of cerium(IV) in H2SO4 (𝐸𝑜 = 1.44 V), HNO3 (𝐸𝑜 = 1.61 V) or HCl (𝐸𝑜 = 1.28 V) [30]. The greater oxidation potential of cerium(IV) in perchloric acid overcomes both the slowness of the oxidation process and the inexact stoichiometry encountered in other acids. The solutions of cerium(IV) in hydrochloric acid are unstable owing to the oxidation of chloride ions to chlorine gas [31]. The refore, in spectrophotometry, the unreacted Ce4+ was treated with p-DMAB in HClO4 medium to yield formic acid and p-dimethylaminophenol, which upon further oxidation gave the corresponding quinoinemine derivative [32]. The possible reaction scheme involving the formation of coloured chromogen is given in Scheme 1.

818405.sch.001

Optimization of Experimental Variables
The experimental variables which provided accurate and precise results were optimized.

Titrimetry
The reaction was found to be quantitative and stoichiometric in H2SO4 medium. A constant reaction stoichiometry of 1 : 1 [GNC : cerium(IV)] was obtained when 1.0–5.0 mL of 2 M H2SO4 was used in a total volume of 25 mL. Hence 2 mL of 2 M H2SO4 was used as optimum for the reaction between GNC and cerium(IV) giving an overall acidity of 0.1 M with respect to H2SO4, and for the latter’s back titration with iron(II). The reaction time was studied by titrating the unreacted cerium(IV) with iron(II) at different time intervals after addition of oxidant to the acidic solution of GNC. It was found that the reaction yielded a constant stoichimetry in the time range 5 to 15 min, and at the standing time less than 5 min and greater than 15 min, there was no constant and definite reaction stoichiometry. Hence, it is necessary to terminate the reaction at the end of the fifth min by back-titrating the residual cerium(IV) with iron(II).

Spectrophotometry
Perchloric acid (4 M) medium was found necessary for rapid and quantitative reaction between GNC and Cerium(IV) and to obtain maximum and constant absorbance values due to cerium(IV)-p-DMAB reaction product at 460 nm. Therefore, all the solutions (GNC, cerium(IV) and p-DMAB) were prepared in 4 M HClO4 throughout the investigation and the same was maintained as reaction medium. To fix the optimum concentration of Ce4+, different concentrations of oxidant were reacted with a fixed concentration of p-DMAB in HClO4 medium and the absorbance measured at 460 nm. A constant and maximum absorbance resulted with 30 μg mL−1 cerium(IV) sulphate and, hence, different concentrations of GNC were reacted with 1 mL of 300 μg mL−1 cerium(IV) sulphate in HClO4 medium before determining the residual Ce4+  via the reaction scheme illustrated earlier. This facilitated the optimization of the linear dynamic range over which procedure could be applied for the assay of GNC. The reaction between GNC and Ce4+ was complete within 15 min at room temperature (28±2°C). After the addition of p-DMAB, a standing time of 5 min was necessary for the formation of coloured product, and thereafter, the coloured product was stable for more than an hour.

3.1. Method Validation

The proposed methods were validated for linearity, sensitivity, precision, accuracy, selectivity, and recovery.

Linearity and Sensitivity
Over the range investigated (3–10 mg GNC), a fixed stoichiometry of 1 : 1 (GNC : Cerium (IV) sulphate) was obtained in titrimetry which served as the basis for calculations. In spectrophotometry, under optimum conditions a linear relation was found between absorbance and concentration in the ranges given in Table 2 and Beer’s law is obeyed in the inverse manner. Sensitivity parameters such as molar absorptivity and Sandel sensitivity, and limits of detection and quantification calculated as per the current ICH guidelines [23] are compiled in Table 2.

Precision and Accuracy
Intraday precision and accuracy of the proposed methods were evaluated by replicate analysis (𝑛=5) of calibration standards at three different concentration levels on the same day. Interday precision and accuracy were determined by assaying the calibration standards at the same concentration levels on five consecutive days. Precision and accuracy were based on the calculated relative standard deviation (RSD, %) and relative error (RE, %) of the found concentration compared to the theoretical one, respectively (Table 3).

Selectivity
The proposed methods were tested for selectivity by placebo blank and synthetic mixture analyses. A convenient aliquot of placebo blank solution prepared as described earlier was subjected to analysis by titrimetry and spectrophotometry according to the recommended procedures. In both the cases, there was no interference by the inactive ingredients.
A separate experiment was performed with the synthetic mixture. The analysis of synthetic mixture solution prepared above yielded percent recoveries in the range 102.7–105.4% with standard deviation of 1.31–3.15. The results of this study indicated that the inactive ingredients did not interfere in the assay. These results further demonstrate the accuracy as well as the precision of the proposed methods.

Robustness and Ruggedness
To evaluate the robustness of the methods, reaction time and H2SO4 concentrations were slightly altered with reference to optimum values in titrimetry. However, in spectrophotometry, the reaction time and volume of p-DMAB were altered. To check the ruggedness, analysis was performed by four different analysts, and on three different burettes (titrimetry) or cuvettes by the same analyst. The robustness and the ruggedness were checked at three different drug levels. The intermediate precision, expressed as RSD (%), which is a measurement of robustness and ruggedness, was within the acceptable limits (0.72–3.74%) as shown in Table 4.

Applicability of the Proposed Methods
The proposed methods were successfully applied to the determination of GNC in pharmaceutical preparations. The results obtained by the proposed methods were compared to those of the reference method [5] by applying Student’s 𝑡-test for accuracy and 𝐹-test for precision. The results (Table 5) show that the Student’s 𝑡- and 𝐹 values at 95% confidence level are less than the theoretical values, which confirmed that there is no significant difference in the performance of the proposed methods and the reference method with respect to accuracy and precision.

Recovery Studies
The accuracy and validity of the proposed methods were further ascertained by performing recovery studies. Preanalysed tablet powder was spiked with pure GNC at three concentration levels (50, 100, and 150% of that in tablet powder) and the total was found by the proposed methods. In all cases, the added GNC recovery percentage values ranged between 101.7 and 109.7% with standard deviation of 0.54–2.42 (Table 6) indicating that the recovery was good and that the coformulated substance did not interfere in the determination.

4. Conclusions

The proposed titrimetric and spectrophotometric methods using Ce(IV)SO4 have suitable performance characteristics for application in the determination of ganciclovir. In particular, the titrimetry is much simpler in technique, more rapid than all the methods reported so far for ganciclovir. The proposed spectrophotometric method employs mild working conditions without heating or extraction and as sensitive as many reported methods. The methods are also useful due to high tolerance limit for common excipients found in drug formulations. Hence, these advantages encourage the application of the proposed methods in routine quality control analysis of ganciclovir in pharmaceutical industries.

Acknowledgment

The authors thank SD Fine Chem. Ltd., India, for gifting pure GNC. Three of the authors P. J. Ramesh, C. M. Xavier, and K. B. Vinay, thank Jubilant Life Sciences, Nanjangud, Mysore, for kind permission to pursue Ph.D. degree.