All other solvents used for analytical work were of HPLC grade an

All other solvents used for analytical work were of HPLC grade and purchased form Merck, Mumbai, India. The patches were prepared initially by four selected permeation enhancers (Oleic acid, Oleyl alcohol, Transcutol

P and Isoproplyl myristate) with drug in Durotak 9301. The cumulative in-vitro drug release upto 8 h was investigated for the prepared patches. The learn more permeation enhancer which has shown highest release was evaluated with DT 900A ( Table 1). Patches were prepared by using solvent casting method. Laboratory coating machine (Laboratory Drawdown Coater-SLDC-100, Shakti Pharmatech, Ahmedabad, India) was used for casting the polymeric blend in patch fabrication. The coating thickness was fixed at 700 μm in order to obtain a patch of thickness

of 500 μm. Coated backing membrane was dried in oven for 60 min at 50 °C. Dried matrix was covered Gemcitabine with PET release liner. Patches were cut in 3.14 cm2 size by using die cutter and stored for the further analysis. The concentration of drug and other excipient were shown in Table 1. The prepared patches were analyzed for adhesive property by invert probe tack test, shear stress test and 90° peel test. The tack test was performed by Invert probe tack tester instrument (mfg. by Cheminstruments Inc.). The shear test was performed according to PSTS-7 procedure by using RT-100 Shear Tester (mfg. by Cheminstruments Inc.). The peel test was performed using peel strength testing machine. The resulted peel value obtained in gram force/2.5 cm2 was converted to N/2.5 cm2. 5 The results were compared against the peel, tack and shear value of Nupatch (Marketed transdermal product of diclofenac by Zydus Cadila, India). Skin hairs of ten to twelve week old male albino rats (250 g) were removed by clippers and full-thickness of rat skin was surgically removed. Epidermis layer was isolated from whole skin and then carefully cleaned with normal saline. Finally fat tissue adhered all to skin was removed by soaking the skin for 30 min in PBS buffer and dried under the vacuum. Dried epidermal

layers were stored in the desiccators until further use. Only the abdomen area was cut from it and square piece used for permeation experiment. Protocol for the use of animal for the above experiment was approved from the Institutional Animal Ethics Committee, Noble Group of Institutions, Junagadh.6 Human cadaver skin (epidermal part) from the chest, back, and abdominal regions were provided by the Parul Institute of Ayurveda (Baroda, India). The skin samples were stored at −20 °C and thawed at room temperature prior to use.7 In-vitro rat skin permeation studies were performed using the modified Franz diffusion cells at 37 °C. Rat skin sample was mounted between donor and receptor compartment. Stratum corneum was faced upward on the donor compartment. FVS patch was applied on the stratum corneum of the skin and receptor compartment was filled with 20 ml of PBS (Phosphate Buffer Saline) pH 6.

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