Int J Pharm Pharm Sci, Vol 7, Issue 3, 191-197Original Article
RP-HPLC METHOD FOR SIMULTANEOUS ESTIMATION AND STABILITY INDICATING STUDY OF METFORMIN AND LINAGLIPTIN IN PURE AND PHARMACEUTICAL DOSAGE FORMS
MALLIKARJUNA RAO. N*1, GOWRI SANKAR D2
1Research scholar, Department of Pharmaceutical Sciences, Jawaharlal Nehru Technological University, Kakinada, Andhra Pradesh, India, 2Professor & HOD, Department of Pharmaceutical Analysis & Quality Assurance, University College of Pharmaceutical Sciences, Andhra University, Visakhapatnam, Andhra Pradesh, India.
Email: mallimpharmmba@gail.com
Received: 07 Oct 2014 Revised and Accepted: 29 Oct 2014
ABSTRACT
Objective: The objective of this study was to develop a simple, efficient, specific, precise and accurate Reverse phase High Performance liquid chromatography method for the simultaneous estimation of Metformin and Linagliptin Pharmaceutical Dosage form.
Methods: The separation method was carried out using reverse phase C18 column, Inertsil ODS – 3V (250 mm x 4.6 mm x 5μm). The mobile phase used was a mixture of Phosphate buffer (1.625 g of Potassium Di Hydrogen Ortho Phosphate and 0.3 g of Di Potassium Hydrogen Ortho Phosphate in 550 ml water) pH 4.5 and Acetonitrile in the ratio of 60:40 (v/v) at isocratic mode. The flow rate was 1.0 mL/min, column temperature was 30°C and eluents were monitored at 280 nm using waters 2695 alliance HPLC instrument equipped with the Waters 2998 PDA detector and Empower 2 software.
Results: With the optimized method, the retention times of Metformin and Linagliptinwere found to be 3.048 and 4.457 respectively, with theoretical plate count and asymmetry as per the limits. The method has shown a good linearity in the concentration range of 500-3000µg/ml from Metformin and 2.5-15µg/mL for Linagliptin with Regression coefficient (R2) of 0.99 and 0.99. The percentage assays were found to be 99.28% and 99.54% respectively for Metformin and Linagliptin. The method was found to be accurate (with percentage mean recoveries 100% for Metformin HCl and 100% for Linagliptin), precise, robust, stable and Degradation studies are conducted under various conditions.
Conclusion: The proposed method was validated in accordance with ICH guidelines and hence, can be successfully applied to the simultaneous estimation of Metformin and Linagliptin tablet formulations.
Keywords: Metformin and Linagliptin, Simultaneous estimation, Reverse phase HPLC, Validation, Degradation studies.
INTRODUCTION
Metformin HCl is an oral hypoglycemicdiabetic drug which comes under the class Biguanides. It is chemically 1, 1-Dimethyl biguanide monohydrochloride. It is the first line drug for treating Type-2 Diabetes mellitus. Metformin acts by suppressing hepatic gluconeogenesis and glucose output from the liver. It is official in USP-2010, BP-2012, and IP-2007 [1-3]. It is the first line drug of choice for the treatment of type 2 diabetes, particularly in overweight or obese people and those with normal kidney function. Metformin activates AMP-activated protein kinase (AMPK), a liver enzyme that plays an important role in insulin signaling, whole body energy balance and metabolism of glucose and fats. Metformin is an anti-diabetic agent [4, 5]. Activation of AMPK is required for metformin’s inhibitory effect on the production of glucose by liver cells. The chemical structure of Metformin is shown in fig. 1.
Fig. 1: Structure of Metformin
Linagliptin is described chemically as 1H-Purine- 2,6-Dione, 8-[(3R) -3-amino-1-piperidinyl] -7-(2-butyn-1- yl) -3,7-dihydro-3-methyl-1-[(4-methyl-2-quinazolinyl) methyl] -The empirical formula is C ₂₅H₂₈N₈O₂. The structural formula is shown in fig (2). Linagliptin is a white to yellowish or only slightly hygroscopic solid substance. It is very slightly soluble in water (0.9 mg mL-1). Linagliptin is soluble in methanol (CA. 60 mg mL-1), sparingly soluble in ethanol (CA. 10 mg mL-1), very slightly soluble in isopropanol (<1 mg mL-1), and very slightly soluble in acetone (CA. 1 mg mL-1). Linagliptin is an oral drug that reduces blood sugar (glucose) levels in patients with type 2 diabetes. Linagliptin is a member of a class of drugs that inhibit the enzyme, DI peptidyl peptidase-4 (DPP-4). Following a meal, insertion hormones such as glucagon-like peptide-1 (GLP-1) and glucose-dependent insulin tropic polypeptide (GIP) are released from the intestine, and their levels increase in the blood. GLP-1 and GIP reduce blood glucose by increasing the production and release of insulin from the pancreas. GLP-1 also reduces blood glucose by reducing the secretion by the pancreas of the hormone, glucagon, a hormone that increases the production of glucose by the liver and raises the blood level of glucose. The net effect of increased release of GLP-1 and GIP is to reduce blood glucose levels. Linagliptin inhibits the enzyme, DPP-4, that destroys GLP-1 and GIP and thereby increases the levels and activity of both hormones. As a result, levels of GLP-1 and GIP in the blood remain higher, and blood glucose levels fall. Linagliptin reduces blood glucose levels by inhibiting DPP-4 and increasing the levels of GLP-1 and GIP [6-8]. The chemical structure of Linagliptin is shown in fig. 2.
Fig. 2: Structure of Linagliptin
For the simultaneous estimation of drugs present in multicomponent dosage forms, HPLC method is considered to be most suitable for this is a powerful and rugged method. Many Methods have been reported in the literature for the estimation of Metformin Hydrochloride [9-19] and Linagliptin [7, 8, 20-23] individually and in combination. However, there is no simple method with shorter run times has been reported for the simultaneous estimation of Metformin Hydrochloride with Linagliptin. The present investigation was aimed at developing a fully validated RP-HPLC method for the simultaneous estimation of Metformin and Linagliptin in pure and pharmaceutical dosage forms that is more economical, simple and accurate than the previous methods.
MATRIALS AND METHODS
Instruments used
The chromatographic determination was performed on waters 2695 alliance HPLC instrument equipped with the waters 2998 PDA detector and Empower 2 software. The different columns were used during method trials such as Inertsil ODS-3V C18column (250 mm×4.6 mm, 5μ particle size), Boston C18 (150 mmX4.6 mm, 5μ), Zodiac C18 (250 mm×4.6 mm, 5μ), etc. Other equipment used were Schimadzu electronic balance AY220, Global Digital pH meter DPH 500, ultrasonic cleaner (Frontline FS 4, Mumbai, India).
Chemicals and reagents
Standard gift samples of Metformin Hydrochloride and Linagliptinwere obtained from Lara drugs Pvt. Ltd., Hyderabad, India. Marketed formulation of combination was purchased from local markets. Acetonitrile, Methanol and water were purchased from HPLC grade was purchased from E. Merck (India) Ltd., Mumbai. Potassium Di Hydrogen Phosphate and Di PotassiumHydrogen Phosphate were purchased from E. Merck, Mumbai, India. All the solvents and reagents were of HPLC grade.
Preparation of standard solution
Accurately weighed standards of Metformin HCl (2000 mg) andLinagliptin (10 mg) were weighed accurately 2000mg of Metformin and 10 mg of Linagliptinwas transferred into 50 ml of volumetric flask dissolved and diluted to volume with the mobile phase and sonicated for 15 min. Pipette out 5 ml of this solution into 25 ml volumetric flasks and make up the volume with the mobile phase.
Preparation of sample solution
Twenty tablets were weighed (average weight 2000 mg) and powdered using mortar and pestle. The quantity of powder equivalent to 500 mg of Metformin HCl and Linagliptini. e., 2000 mg was transferred to a 50 ml volumetric flask. The content was dissolved in the mobile phase, sonicated for15 minutes to dissolve the drug as completely as possible. The solution was then filtered through 0.45μNylon disposable Syringe filter. The volume was then made to mark with the mobile phase. This is the standard stock solution. From the standard stock solution, an aliquot of 5 ml solution was transferred to a 25 ml volumetric flask and diluted to mark with the mobile phase
RESULTS AND DISCUSSION
Method development
Initially, many method trials were performed using different mobile phases, different columns, and varying chromatographic conditions in an attempt to obtain the best separation and resolution between Metformin HCl and Linagliptinas shown in fig. 3. The finalized method involved the use of a mixture of Phosphate buffer (1.625 g. of Potassium Di Hydrogen Ortho Phosphate and 0.3 g of Di Potassium Hydrogen Ortho Phosphate in 550 ml water); pH 4.5 and Acetonitrile in the ratio of 60:40 (v/v) as the mobile phase at isocratic mode and eluents were monitored at 280 nm using UV-Visible spectrophotometer as the detector allowing the adequate separation of both the compounds using the column Inertsil ODS - 3V C18 (250 mm x 4.6 mm x 5μm particle size) at a flow rate of 1.0 ml/min and column temperature 30°C. Sample injection volume was 1.0 ml/minas shown in fig. 4.
Assay procedure
With the optimized chromatographic conditions, a steady baseline was recorded, the mixed standard solution was injected five times and the chromatograms were recorded. This procedure was repeated for the sample solution too. The averages of peak areas were determined for standard and sample solutions. The concentration of the drug was calculated using the following formula
The results are described in table 1.
Fig. 3: Typical chromatogram for the trial
Fig. 4: Typical chromatogram for the standard
Table 1: Assay results of Metformin and Linagliptin
| Drug | % Assay |
| Metformin | 99.28 |
| Linagliptin | 99.54 |
Method validation [20-23]
System suitability
The suitability of the chromatography system was tested before each stage of validation. Six replicates of working standard solution are injected and the chromatograms are recorded. The % Relative Standard Deviation (%RSD) of retention times, asymmetry, theoretical plate count and of peak areas (should not be more than 2%) was determined as shown in table 2 and fig. 5.
Fig. 5: Typical chromatogram for the standard
Table 2: System suitability parameters
| Parameters | Metformin | Linagliptin |
| Retention time | 3.048 | 4.457 |
| Resolution | - | 7.970 |
| Theoretical plates | 6782 | 8231 |
| Tailing | 1.147 | 1.096 |
Accuracy
To the pre-analyzed sample solution, a known amount of standard solution (usually 5-20%) was spiked at three different levels (50%, 100%, and 150%). These solutions were injected in three replicates and Percentage Mean Recoveries are determined for Metformin and Linagliptin which should lie between 98-102%. The results are described in table 3, 4 and fig. 6, 7 and 8.
Table 3: Accuracy for Metformin
| Spiked level | Sample weight | Sample area | µg/ml added | µg/ml found | % recovery | Mean |
| 50% | 2045.00 | 4520363 | 3958.065 | 3958.42 | 100 | 100 |
| 50% | 2045.00 | 4525808 | 3958.065 | 3958.42 | 100 | |
| 50% | 2045.00 | 4524672 | 3958.065 | 3958.42 | 100 | |
| 100% | 4090.88 | 9055238 | 7917.832 | 7930.00 | 100 | 100 |
| 100% | 4090.88 | 9056005 | 7917.832 | 7930.00 | 100 | |
| 100% | 4090.88 | 9053824 | 7917.832 | 7930.00 | 100 | |
| 150% | 6135.0 | 13518335 | 11874.194 | 11838.50 | 100 | 100 |
| 150% | 6135.00 | 13516919 | 11874.194 | 11838.50 | 99 | |
| 150% | 6135.00 | 13568589 | 11874.194 | 11838.50 | 100 |
Table 4: Accuracy for Linagliptin
| Spiked level | Sample weight | Sample area | µg/ml added | µg/ml found | % recovery | Mean |
| 50% | 2045.00 | 4358197 | 19.990 | 19.96 | 100 | 100 |
| 50% | 2045.00 | 4356218 | 19.990 | 19.95 | 100 | |
| 50% | 2045.00 | 4352141 | 19.990 | 19.93 | 100 | |
| 100% | 4090.88 | 8707432 | 39.989 | 39.88 | 100 | 100 |
| 100% | 4090.88 | 8700880 | 39.989 | 39.85 | 100 | |
| 100% | 4090.88 | 8706209 | 39.989 | 39.87 | 100 | |
| 150% | 6135.0 | 13056602 | 59.971 | 59.80 | 100 | 100 |
| 150% | 6135.00 | 13022412 | 59.971 | 59.64 | 99 | |
| 150% | 6135.00 | 13048584 | 59.971 | 59.76 | 100 |
Fig. 6: chromatogram of 50% accuracy level |
Fig. 7: chromatogram of 100% accuracy level |
Fig. 8: chromatogram of 150% accuracy level |
Precision
The precision of the method (Intra-day variation) was determined by repeatedly injecting the sample solution (8mg/ml of Metformin HCl and 0.5mg/ml Linagliptin) six times. The retention times and peak areas of six replicates are recorded. The precision is expressed as the % RSD of Peak areas and it should not be more than 2%. The results are described in table 5 and 6.
Table 5: Intraday precision
| S. No. | Sample weight | Metformin | Linagliptin | % Assay (metformin) | % Assay (linagliptin) |
| 1 | 4090.88 | 9058615 | 8707008 | 99 | 100 |
| 2 | 4090.88 | 9055892 | 8706154 | 99 | 100 |
| 3 | 4090.88 | 9058196 | 8705139 | 99 | 100 |
| 4 | 4091.88 | 9056969 | 8701982 | 99 | 100 |
| 5 | 4090.88 | 9053353 | 8700572 | 99 | 100 |
| 6 | 4090.88 | 9054070 | 8703774 | 99 | 100 |
| Average Assay: | 99 | 100 | |||
| SD | 0.02 | 0.03 | |||
| %RSD | 0.02 | 0.03 |
Table 6: Interday Precision
| S. No. | Sample weight | Metformin | Linagliptin | % Assay (metformin) | % Assay (linagliptin) |
| 1 | 4091 | 9058245 | 8702651 | 100 | 100 |
| 2 | 4091 | 9057486 | 8703148 | 100 | 100 |
| 3 | 4091 | 9058954 | 8705246 | 100 | 100 |
| 4 | 4091 | 9056847 | 8701431 | 100 | 100 |
| 5 | 4091 | 9055078 | 8706054 | 100 | 100 |
| 6 | 4091 | 9059834 | 8704297 | 100 | 100 |
| Average Assay: | 9057740.7 | 8704297 | 100 | 100 | |
| SD | 1677 | 2234 | 0.02 | 0.03 | |
| %RSD | 0.02 | 0.03 |
Linearity
The calibration curve was constructed by plotting peak area against concentration of solutions. Metformin and Linagliptin were found to be linear in the concentration range of 500-3000µg/mL (25 % to 150%) and 2.5-15µg/mL (25% to 150%) respectively. The results show that an excellent correlation exists between areas and concentration of drugs within the concentration range indicated above. The results of linearity were represented in tables 7. And the results for calibration curves are given in fig. 9 & 10.
Table 7: Linearity of Metformin and Linagliptin
| Linagliptin and metformin Con. c% | Metformin area | Metformin µg/ml | Linagliptin area | Linagliptin µg/ml |
| 25 | 2336359 | 500 | 2148043 | 2.5 |
| 50 | 4524579 | 1000 | 4354630 | 5 |
| 75 | 6788434 | 1500 | 6536100 | 7.5 |
| 100 | 9057249 | 2000 | 8704856 | 10 |
| 125 | 11379261 | 2500 | 10866198 | 12.5 |
| 150 | 13583129 | 3000 | 13086472 | 15.00 |
Fig. 9: Linearity Curve for Metformin
Robustness
The robustness of the method is determined under normal operating conditions different conditions such as change in flow rate and detection wave length. 10 μl of standard and sample solutions are injected by varying wavelength (282, 284, 286 nm) and the flow rate (0.8 ml/min, 1.0 ml/min, 1.2 ml/min) and the chromatograms are recorded and changes in parameters are observed. The results are shown in table 8 and 9
Fig. 10: Linearity curve for Linagliptin
Table 8: Robustness for Metformin
| S. No. | Sample name | Change | RT | Area | Tailing | Plate count |
| 1 | Flow1 | 0.8 ml | 3.810 | 11279449 | 1.211 | 7134 |
| 2 | Flow 1 | 0.8 ml | 3.805 | 11359450 | 1.210 | 6800 |
| 3 | Flow 1 | 0.8 ml | 3.804 | 11325956 | 1.230 | 6935 |
| 4 | Flow 2 | 1.2 ml | 2.546 | 7368090 | 1.158 | 5916 |
| 5 | Flow 2 | 1.2 ml | 2.544 | 7343308 | 1.179 | 5989 |
| 6 | Flow 2 | 1.2 ml | 2.542 | 7329988 | 1.191 | 6128 |
| 7 | Temp 1 | +5°C | 3.048 | 8967960 | 1.194 | 6494 |
| 8 | Temp 1 | +5°C | 3.052 | 8962415 | 1.173 | 6423 |
| 9 | Temp 1 | +5°C | 3.047 | 8971075 | 1.256 | 6581 |
| 10 | Temp 2 | -5°C | 3.041 | 8956081 | 1.158 | 6602 |
| 11 | Temp 2 | -5°C | 3.034 | 8922707 | 1.198 | 6732 |
| 12 | Temp 2 | -5°C | 3.045 | 9003965 | 1.155 | 6679 |
Forced degradation studies
Degradation studied is performed under different conditions like acid, base, peroxide, photo and Thermal. In each degradation study for both Metformin and Linagliptin it was observed that purity angle is less than the threshold value, it indicated the no interference of degradants with the drug peaks so the peak was said to be pure. Degradation studies reveal that the developed method was stability indicating hence, this method can easily and conveniently adopt for routine quality control analysis of Metformin and Linagliptin in pure and its pharmaceutical dosage forms. It was observed that there was marked degradation in the chromatograms, and the data given in Tables 10&11. Purity plots for Metformin (Fig.11a-11e) and Linagliptin (Fig.12a-12e) were shown.
Table 9: Robustness for Linagliptin
| S. No. | Sample name | Change | RT | Area | Tailing | Plate count |
| 1 | Flow 1 | 0.8 ml | 5.519 | 11117649 | 1.169 | 9036 |
| 2 | Flow 1 | 0.8 ml | 5.504 | 11133699 | 1.186 | 9236 |
| 3 | Flow 1 | 0.8 ml | 5.501 | 11149431 | 1.208 | 8958 |
| 4 | Flow 2 | 1.2 ml | 3.694 | 7214335 | 1.134 | 7607 |
| 5 | Flow 2 | 1.2 ml | 3.682 | 7215805 | 1.144 | 7584 |
| 6 | Flow 2 | 1.2 ml | 3.678 | 7191727 | 1.154 | 7446 |
| 7 | Temp 1 | +5°C | 4.403 | 8828575 | 1.143 | 8352 |
| 8 | Temp 1 | +5°C | 4.419 | 8802088 | 1.148 | 8290 |
| 9 | Temp 1 | +5°C | 4.417 | 8821620 | 1.182 | 8012 |
| 10 | Temp 2 | -5°C | 4.363 | 8832817 | 1.185 | 8753 |
| 11 | Temp 2 | -5°C | 4.343 | 8813283 | 1.177 | 8447 |
| 12 | Temp 2 | -5°C | 4.369 | 8872802 | 1.146 | 8560 |
Table 10: degradation studies for metformin
| Mode of degradation | Conditions | Sample weight | Area | % Assay | Purity Angle | % Deg. | Purity Threshold |
| Control | No treatment | - | - | - | - | - | - |
| Acid degradation (5N HCl) | 40°C/5 minutes | 4091 | 7287975 | 80 | -19 | 0.746 | 0.891 |
| Alkali degradation (1N NaOH) | 80°C/1 hours | 4091 | 7681508 | 84 | -15 | 0.818 | 1.062 |
| Peroxide (30%W/V H2O2) | 80°C/10 minutes | 4091 | 7790730 | 85 | -14 | 0.702 | 0.994 |
| Light (200watts hrs/min) | 105°C/72 hours | 4091 | 8593479 | 94 | -5 | 0.961 | 1.085 |
| Heat (105°C/72hr) | 25°C/72 hours | 4091 | 8544169 | 94 | -5 | 0.743 | 0.910 |
Table 11: Degradation studies for Linagliptin
| Mode of degradation | Conditions | Sample weight | Area | % Assay | % Deg. | Purity Angle |
Purity Threshold |
| Control | No treatment | - | - | - | - | - | - |
| Acid degradation (5N HCl) | 40°C/5 minutes | 4091 | 6973352 | 80 | -20 | 9.048 | 14.724 |
| Alkali degradation (1N NaOH) | 80°C/1hour | 4091 | 7367552 | 84 | -16 | 9.563 | 16.016 |
| Peroxide (30%W/V H2O2) | 80°C/10 minutes | 4091 | 7666328 | 88 | -12 | 9.328 | 13.864 |
| Light (200watts hrs/min) | 105°C/72 hours | 4091 | 8068628 | 92 | -8 | 9.109 | 13.038 |
| Heat (105°C/72hr) | 25°C/72 hours | 4091 | 8031372 | 92 | -8 | 8.275 | 15.559 |
Purity Plots for Metformin
| Fig. 11a: Acid degradation | Fig.11 b: Alkali degradation |
| Fig. 11c: thermal degradation | Fig. 11d: Peroxide degradation |
| Fig. 11e: Photolytic degradation |
Purity Plots for Linagliptin
| Fig. 12a: Acid degradation | Fig. 12b: Alkali degradation |
| Fig. 12c: photolytic degradation | Fig. 12d: Thermal degradation |
| Fig. 12e: Peroxide degradation |
CONCLUSION
The developed RP-HPLC method was developed and validated as per ICH guidelines in terms of specificity, accuracy, precision, linearity, robustness, limit of detection and limit of quantitation for the simultaneous quantitative estimation of Metformin and Linagliptin. The correlation coefficients were greater than 0.99 for both the drugs. The precision results were good enough to say that the method developed is precise and reproducible.
Accuracy studies revealed that mean recoveries after spiking experiments were between 99 and 101%, indicative of accurate method. Degradation studies reveal that the developed method was stability indicating hence, this method can easily and conveniently adopt for routine quality control analysis of Metformin and Linagliptin in pure and its pharmaceutical dosage forms.
ACKNOWLEDGEMENT
Authors are thankful to the Department of Pharmaceutical Sciences, Jawaharlal Nehru Technological University, and Kakinada. And Department of Pharmaceutical Sciences, Andhra University, Visakhapatnam for providing instrumental and analytical support.
CONFLICT OF INTEREST
Declared None
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