Formulation of Convenient, Easily Scalable, and Efficient Granisetron

May 2, 2015 - The prepared nine droppable gels were evaluated in vitro, ex vivo through sheep nasal mucosa, as well as in vivo in comparison to drug ...
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Formulation of convenient, easy scalable and efficient granisetron HCl intranasal droppable gels Howida K. Ibrahim, Nevine S. AbdelMalak, and Sally A. Abdel Halim Mol. Pharmaceutics, Just Accepted Manuscript • DOI: 10.1021/mp500825n • Publication Date (Web): 02 May 2015 Downloaded from http://pubs.acs.org on May 7, 2015

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Formulation of convenient, easy scalable and efficient granisetron HCl intranasal droppable gels. Howida k. Ibrahim*, Nevine S. AbdelMalak, Sally A. Abdel Halim Department of pharmaceutics and industrial pharmacy, Faculty of Pharmacy, Cairo University, Kasr Al-ini street, 11562. Abstract Deacetylated gellan gum and two sodium alginate polymer types were used each at three concentrations in the suitable range for their sol-gel transition. The prepared nine droppable gels were evaluated in-vitro, ex-vivo through sheep nasal mucosa, as well as, in-vivo in comparison to drug solution given intravenously and orally at the same dose. The prepared formulae gelled instantaneously in simulated nasal fluid and the obtained gels sustained their shear thinning and thixotropic behavior up to 48h. Polymer type and concentration had significant effects on the apparent viscosities and the in-vitro release profile of granisetron from the prepared gels. The drug release data best fitted modified Higuchi equation with initial burst and followed Fickian diffusion mechanism. 0.5% gellan gum based formula sustained the in-vitro drug release up to 3h and enhanced the drug permeation without need for an enhancer. The histopatholgical study revealed the safety of the tested formula. Intranasal delivery recorded double the drug bioavailabilty in comparison to the oral route. It had an absolute bioavailability of 0.6539 and the maximum plasma drug concentration reached after 1.5h. The developed formula could be promising for the management of chemotherapy-induced nausea and vomiting regarding its improved bioavailability, patient acceptability and ease of production. Key words: granisetron HCl, droppable gel, intranasal delivery INTRODUCTION Nausea and vomiting are the most upsetting adverse reactions of cancer chemotherapy. Serotonin (5 hydroxytryptamine, 5-HT) was proved to be at least partially responsible for producing those effects. Ligand binding to 5-HT3 receptor type induces nausea and vomiting. Thus Current guidelines propose 5-HT3 receptor blockage as an intervention. (1, 2) Highly potent and selective 5-HT3 receptor antagonists include ondansetron, granisetron and tropisetron. Granisetron is the most selective with consequent less adverse effects. (3, 4) It prevents acute emesis by acting at both periphral (GI tract) and central (medullary chemoreceptor zone) sites. (5) Granisetron proved to be effective and well tolerated as antiemetic in children too. (6) Orally administered granisetron is subjected to hepatic first pass effect. Granisetron HCl is available commercially as oral tablets, as well as, a solution for IV administration. Some trials were conducted for the transdermal delivery of granisetron to overcome the hepatic first pass metabolism. (7-12) A study investigated delivering it as suppository (13) and another through the buccal cavity. (14) Clinical trials in animals and healthy volunteers proved the possibility of delivering granisetron HCl solution through the nasal 1 ACS Paragon Plus Environment

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mucosa with rapid absorption and improved bioavailability in comparison to oral administration. (15, 16) The drug had an excellent safety profile regarding irritation to the nasal mucosa and abnormal changes in clinical laboratory tests. (17) Literature lacks formulation trials of granisetron HCl for the intranasal delivery except for the preparation of freeze-dried microparticles composed of granisetron-cyclodextrin complex and carboxymethylcellulose. (18) This work focused on the solubilization of granisetron base and did not test the drug bioavailability. Intranasal delivery is a convenient alternative to the parenteral route. The high blood supply and permeability of the nasal mucosa guarantee systemic drug delivery. Yet, mucociliary clearance limits the residence time for drug to be absorbed. Droppable gels improve nasal drug absorption. Gellan gum and alginates are biodegradable and non-toxic polysaccharides. Their high water holding capacity and/or mucoadhesive potential make them useful carriers for the nasal cavity without harmful effects. (19, 20) Thus, the aim of this work was to formulate granisetron HCl as intranasal droppable gels for improved patient compliance and enhanced therapeutic effect. The work will investigate different ion activated in situ gelling polymers at different concentrations with and without permeation enhancer. Thorough in-vitro and ex-vivo evaluations will be conducted and the formula of choice will be compared to drug solution given orally and intravenously in experimental animals. METHODS Materials: Granisetron HCl was kindly gifted by Amoun Pharmaceuticals, Egypt, two types of sodium alginate; low and high molecular weights (LMW, HMW), deacetylated gellan gum and acetonitrile (HPLC grade) were purchased from Sigma-Aldrich, St Louis, MO, USA, sodium chloride, potassium chloride and calcium chloride dihydrate (ADWIC Co., Egypt). The simulated nasal fluid was composed of 7.45 mg/ml NaCl, 1.29 mg/ml KCl and 0.32 mg/ml CaCl2·2H2O and pH adjusted at 5.5. Stability of granisetron HCl in nasal mucosa extract Fresh excised nasal sheep mucosa was extracted in normal saline by stirring for 5h. Granisetron was added to 5 ml of the collected extract and kept for 24h at 37 ◦C. The remaining drug content was analyzed using the stability indicating HPLC assay developed by Souri et al. (21) A 75:25 v/v mixture of acetonitrile and 25 mM KH2PO4 was used as the mobile phase. Separation was done using a Nova-Pak C8 column (60Å, 4 µm, 3.9 mmx150 mm, Waters) and detection was performed at 305 nm. A paired t-test was conducted to evaluate the results. Preparation of droppable gels The used polymer concentration ranges were determined based on literature (22, 23), as well as, on preliminary experiments. The three polymers were tested in concentrations ranging from 0.05 to 2%.Three concentrations were selected for each polymer. Sols at the selected concentrations

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should have spontaneous sol-gel transformation and all are less than the concentration leading to a gel without the addition of the nasal fluid. Deacetylated gellan gum sols were prepared in ultrapure water with stirring at 90oC at three concentrations (0.1, 0.2 and 0.5%). The drug was dissolved in the resulting sols after cooling to room temperature as 1% w/v. Alginate sols were prepared by sprinkling the corresponding amounts of either the low or high molecular weight grades in ultrapure water. The sols were left overnight at room temperature and the drug was added by stirring. The alginate sols were prepared at three concentrations, namely, 0.5, 0.75 and 1%. The composition of the prepared formulae is shown in table 1. Gelling and rheological properties Sol-gel transition of the prepared droppable gels was tested visually in simulated nasal fluid. Gellation was tested by mixing at 1: 1 formula to nasal fluid ratio, as well as, by dropping the formulae onto the nasal fluid and vice versa. The obtained gels were kept and observed for 48h post mixing. The rheological properties of the drug loaded formulae were determined using a cone and plate Brookfield viscometer (model HBDV-I, Brookfield Engineering Laboratories, Inc., Middleboro, MA, USA) at 25°C using 1 ml sample aliquots. Apparent viscosity values were measured at different angular velocities (10-100 rpm) with a similar wait before each change in speed. Rheograms were constructed by plotting apparent viscosity values versus angular velocities from 10 to 100 and down back. Measurements were done in duplicate. For comparison, the exponential formula was used and the exponent N (Farrow's constant) was calculated. In-vitro release profile One gram droppable gel samples were filled in dialysis bag (Spectrapor membrane tubing No. 2 Spectrum Medical Industries, USA) and mounted in 100 ml simulated nasal fluid. The test was carried out in United States Pharmacopia XXVIII dissolution apparatus Type II operated at 50 rpm and 37 ±1oC. Aliquots of 1 ml volume were withdrawn up to 3h. The drug content was determined spectrophotometrically after proper dilution. The release efficiency after 3h (RE3h) was measured according to Modi and Tayade (24) as a parameter for the release extent. ANOVA analysis with subsequent Tukey-Kramer multiple comparison test were conducted to study the effect of both polymer type and polymer concentration on the release behavior. The (qs) values were calculated and compared to a (q) value from the studentized range distribution. Tukey confidence limits were also calculated for all pairwise comparisons. Mathematical modeling of the release data from the droppable gels was done using DDSolver (an Excel add-in software package). The adjusted coefficient of determination (2adjusted) was considered for finding the best fit of the release data to the zero order, first order, as well as, Higuchi equation and its modified form describing the initial burst release effect (0). The nontransformed release data were also fitted to the Korsmeyer-Peppas model and its modified form with burst (25) employing Nelder-Mead simplex algorithm. (26) The exponent  values were 3 ACS Paragon Plus Environment

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calculated using the nonlinear least-squares curve-fitting technique and were used for investigating release mechanism. (27) Ex-vivo permeation and local toxicity on sheep nasal mucosa The permeation of the selected droppable gels was assessed through freshly excised sheep nasal mucosa. Hydroxypropyl β-cyclodextrin (10%) was added as an enhancer (28), composition of the tested formulae is shown in table 3. The test was conducted in a modified diffusion cell with diffusional area of 3.14 cm2 and 7 ml receiver chamber capacity. The droppable gels were added to the donor compartment after mixing with nasal fluid at 1: 1 ratio. The permeated drug was received in simulated nasal fluid maintained at 37oC and magnetically stirred at 50 rpm. The whole receptor fluid was replaced at each time interval and analyzed by HPLC. The mean cumulative amount permeated per unit surface area of the nasal mucosa was plotted versus time. The slope of the linear portion of the plot was calculated to represent the steady state flux (Jss). Apparent permeability coefficient (KP) was calculated by dividing the flux by initial concentration of the drug in the donor compartment. Permeation data was subjected to statistical analysis using one way ANOVA and Tukey multiple comparison tests. The effect of the enhancer on the permeation profiles for both formulae was (29) evaluated using the similarity factor. At the end of the permeation test, the used nasal mucosa sections were transferred into 10% formalin solution. They were stained with haematoxylin-eosin and examined under the light microscope (Axiovert 200MAT, Carl Zeiss, Germany) by a pathologist. A control nasal mucosa section was also examined after soaking in nasal fluid for 7h. In-vivo evaluation The pharmacokinetics of granisetron HCl was studied after the administration of a single intranasal dose (1 mg/kg) of the selected droppable gel formula (F9) to six New Zealand albino rabbits (2.94±0.13 kg). The marketed IV Granisetron HCl solution (Emex, Amoun Pharmaceutical Company) was used as the reference, both intravenously and orally at the same intranasal dose in a cross over design. Blood samples were collected from the marginal ear vein at 5, 20, 40 min and 1, 1.5, 2, 3, 4, 5, 6 and 7 h after drug administration. After centrifugation, the plasma was separated and frozen until analysis. Granisetron HCl was measured in plasma applying the previously described HPLC method with slight modifications. (21) The rabbits were fasted overnight with free access to water prior to and during the experiment. The study protocol was reviewed and approved by the Research Ethics Committee of Faculty of Pharmacy, Cairo University. The maximum observed plasma concentration (Cmax) and the time taken to achieve it (Tmax) were obtained directly from the curves. The area under the plasma concentration-time curve up to the last quantified sample (AUC0–7h) was calculated using the trapezoidal rule. The first order terminal elimination rate constant (ke) was estimated by linear regression from the points describing the elimination phase on a log-linear plot. It was used to calculate the AUC0-inf and t1/2. The AUC 0-inf values obtained from the granisetron HCl curves after the administration of the IV and oral solutions, as well as, the nasal droppable gel were used to calculate the absolute bioavailability. 4 ACS Paragon Plus Environment

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The mean pharmacokinetic parameter values were compared using a one-way ANOVA followed by Tukey-Kramer multiple comparison test. A p-value of less than 0.05 was considered significant. RESULTS AND DISCUSSION Stability of granisetron HCl in nasal mucosa extract The remaining granisetron HCl amount after 24h in nasal mucosa extract was 98.54%. It was non-significantly different from the initial added amount (99.21%) indicating high drug stability. Preparation of droppable gels Gellan gum and alginate have been granted regulatory approvals as pharmaceutical excipients and food additives and literature thoroughly investigated their safety for intranasal administration. Gelling and rheological properties Sol-gel transition occurred immediately upon contact with the simulated nasal fluid regardless of the mixing ratio or order (lag time values were less than 10 sec). This rapid gellation is essential to overcome the mucociliary clearance from the nasal cavity. Mucus transit time ranges from 15 to 20 min with a transport rate of 5 mm/min. (30) All the prepared formulae exhibited shear thinning behavior before gellation (N >1, table 1). Polymer type had significant effect on the rheological properties. High molecular weight alginate based systems recorded comparable viscosity values to gellan gum ones, figure 1 (b and c). On the other hand, the viscosities and degrees of pseudoplasticity of low molecular weight alginate based formulae were markedly lower. Their upward and downward curves were almost superimposed showing no thixotropic behavior, figure 1 (a). Increasing polymer concentration markedly increased apparent viscosity and degree of pseudoplasticity. Thixotropy was prominent only for formulae F5, F6 and F9, prepared at the highest concentrations of HMW alginate and gellan gum polymers. Thixotropy will add an advantage to gel-sol-gel behavior during use (eg. spraying or dropping of the sols) and can ensure the formation of a firm reservoir in the nasal mucosa. Viscosity increased significantly after gellation. Similarly, did the pseudoplastic and thixotropy degrees. The rheograms of LMW alginate based formulae had very low apparent viscosities and degrees of pseudoplasticity even in presence of nasal fluid ions. The obtained rheograms after sol-gel transition were stable for more than 48h for the three polymers, data are not shown. In-vitro release profile Figure 2 (a, b and c) shows the in-vitro release profile of granisetron from the prepared droppable gels while the calculated RE3h values are listed in table 1. Results of ANOVA test proved significant differences between the mean RE3h values at level of significance α=0.05. Post-hoc analysis was conducted to determine which means differ. The calculated (qs) values were larger than the qcritical value (4.956) for all pairs proving significant differences of release extent among all formulae. Only formulae F2 and F4 had non-significantly different RE3h values (qs = 4.795), table 1.

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Statistical analysis showed that changing polymer type and polymer concentration significantly affected the in-vitro drug release from the prepared droppable gels. The polymers can be arranged in an ascending order according to their ability to sustain granisetron release as LMW alginate < HMW alginate < gellan gum. Low molecular weight alginate based formulae released 100% of their loaded drug within 30-120 min. The low viscosity could be the cause for this poor drug release sustainment. This duration was longer for HMW alginate based formula (120-240 min). Only 0.5% gellan gum formula succeeded in controlling the drug release up to 360 min. Increasing polymer concentration significantly decreased the release rate and extent. This could be rationalized in terms of the marked increase in viscosity at higher polymer concentrations. The release data of droppable gel formula F3, F6 and F9 (showing controlled drug release) were fitted into different kinetic models. The highest 2adjusted values were obtained with modified Higuchi equation describing the initial burst release effect. The outputted burst and T90% values are shown in table 2. The release data better fitted the Korsmeyer-Peppas model rather than its modified form with burst. The (n) exponent values ranged from 0.306 to 0.341 supporting the diffusion mechanism, table 2. The drug release is controlled by diffusion through the threedimensional structures of gellan gum and alginate after sol-gel transition. In presence of cations, gellan gum chains bind forming double-helical junction zones, which further aggregate in presence of water giving 3-D networks. (31) Sodium alginate forms 3-D ionotropic hydrogel matrices through the interaction of its guluronic acid moieties with calcium ions. Formulae F6 and F9 recorded significantly lower burst and higher T90% values than those of F3 and were selected for further investigations. Ex-vivo permeation and local toxicity on sheep nasal mucosa Sheep nasal mucosa was selected because of its human-like histology. (32) Gellan gum based formula (F9) recorded significantly higher flux than that of alginate formula (F6), figure 4 and table 3. Hydroxypropyl β-cyclodextrin showed no permeation enhancing effects of granisetron HCl from both formulae. The calculated similarity factors were 98.85 and 97.32 for formulae F6 and F9 with and without enhancers, respectively. The polar nature and the low molecular weight of the drug (348.9 Da) suggest crossing the nasal epithelial membrane by paracellular route. (33) Figure 4(a-d) shows that the structure of the mucosa was well preserved after 7h exposure to the drug loaded gels with and without enhancer. No signs of irritation or toxicity were detected. Histological sections of the control and the treated nasal mucosa were similar in tissue architecture. Based on the obtained flux and the calculated ( f2) values, formula F9 without enhancer was selected for calculating drug pharmacokinetics in rabbits. In-vivo evaluation Figure 5 shows the plasma drug concentration versus time curves after nasal, oral and I.V administration of granisetron. The calculated pharmacokinetic parameters are shown in table 3. Intranasal administration of granisetron HCl significantly improved the drug absorption rate and extent compared to the oral route. This is due to escaping the hepatic first pass metabolism. Formulating the drug as a droppable gel via the nasal route significantly increased its t1/2 in body 6 ACS Paragon Plus Environment

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compared to the oral solution. This could be due to the long residence time in the nasal cavity and the prolonged in-vitro release profile of the drug from the gels. The maximum plasma concentrations were reached after 1.5 and 2.5h for intranasal and oral routes, respectively. Blum et al. (34) reported that the time to reach peak concentration was 3h after administration of oral tablets in “healthy individuals.; PDR, 2005)”. The intranasal droppable gel recorded an absolute relative bioavailability of 0.6539. Its measured Cmax, AUC0-7 and AUC0-inf were significantly lower than the corresponding parameters after IV administration of the drug solution. On the other hand, Jong Soo Woo (16) reported that the bioavailability of granisetron solution following nasal administration was comparable to that following IV administration of the same dose in rats, regarding their Cmax and elimination halflife. This could be justified in terms of the different drug dosage forms. Conclusion Granisetron HCl was successfully formulated as a droppable gel for intranasal administration. The drug was stable and did not show histological evidence of irritation or toxicity. Droppable gels combine the advantages of accurate dosing and easy administration of solutions and the longer contact time and prolonged release profile of gels. The release profile was tailored by changing the polymer type and concentration. Intranasal administration doubled the granisetron bioavailability in comparison to the oral route. It is more convenient and easier to administer in relation to the IV injection. The maximum drug concentration in plasma reached after 1.5h which suggests dosing 1h before radiation therapy. Acknowledgements and funding Authors would like to thank Dr. Shady Elia Anis, M.D., lecturer of pathology, Cairo University for help in conducting the local toxicity test. This research received no specific grant from any funding agency in the public, commercial, or not-for-profit sectors. References 1. Gan, T.J. Selective serotonin 5-HT3 receptor antagonists for postoperative nausea and vomiting: are they all the same?. CNS Drugs. 2005,19(3), 225-38. 2.Tan, M. Granisetron: new insights into its use for the treatment of chemotherapy-induced nausea and vomiting. Expert Opin Pharmacother. 2003, 4(9),1563-71. 3.Freeman, A.J, Cunningham, K.T., Tyers, M.B. Selectivity of 5-HT3 receptor antagonists and anti-emetic mechanisms of action. Anti-Cancer Drugs 1992, 3(2), 79-85. 4.Marr, H.E., Davey, P.T., Bartlett, A.J. Emerging differences between 5-HT3 receptor antagonists. Anti-cancer Drugs 1991, 2, 513-518. 5.Feyer, P., Seegenschmiedt, M.H., Steingraeber, M. Granisetron in the control of radiotherapyinduced nausea and vomiting: a comparison with other antiemetic therapies. Support Care Cancer. 2005, 13(9), 671-8. 6.Yarker, Y.E., McTavish, D. Granisetron: an update of its therapeutic use in nausea and vomiting induced by antineoplasmic therapy. Drugs. 1994, 48, 761-793. 7.Chaturvedula, A., Joshi, D.P., Anderson, C., Morris, R., Sembrowich, W.L., Banga, A.K., Dermal, subdermal, and systemic concentrations of granisetron by iontophoretic delivery. Pharm. Res. 2005, 22, 1313–1319. 7 ACS Paragon Plus Environment

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8.Zheng, W.W., Zhao, L., Wei, Y.M., Ye, Y., Xiao, S.H., Preparation and the in-vitro evaluation of nanoemulsion system for the transdermal delivery of Granisetron hydrochloride. Chem. Pharm. Bull. 2010, 58, 1015–1019. 9.Zhao, N., Cun, D., Li, W, et al. , In-vitro percutaneous absorption enhancement of granisetron by chemical penetration enhancers. Drug Dev Ind Pharm., 2013, 39(4), 561-8. 10. Zheng, W.W., Zhao, L., Wei, Y.M., et al. Preparation and the in-vitro evaluation of nanoemulsion system for the transdermal delivery of granisetron hydrochloride. Chem Pharm Bull (Tokyo) 2010, 58(8),1015-9. 11. Cázares-Delgadillo, J., Ganem-Rondero, A., Quintanar-Guerrero, D., et al. Using transdermal iontophoresis to increase granisetron delivery across skin in-vitro and in vivo: effect of experimental conditions and a comparison with other enhancement strategies. -U.S. Eur J Pharm Sci., 2010, 39(5), 387-93. 12. Mogal, V., Puranik, P. Enhanced Transdermal Delivery of Granisetron Hydrochloride via Ethosomes, Journal of Medical and Pharmaceutical Innovation, 2013, 1 (1), 24-30. 13. Slunkhe, N.H., Jadhav, N.R., Mali, K.K., Dias, R.J., Ghorpade, V.S., Yadav, A.V., Mucoadhesive microspheres based suppository containing granisetron HCl for management of emesis in chemotherapy. Journal of Pharmaceutical Investigation, 2014, 44, 253-263. DOI 10.1007/540005-014-0123.6 14. Ahmed, S., El-Setouhy, D.A., Badawi, A.A., El-Nabarawi, M.A., Provesicular granisetron hydrochloride buccal formulations: In vitro evaluation and preliminary investigation of in vivo performance, European Journal of Pharmaceutical Sciences. 2014, 60, 10–23. 15. Hussain, A. A., Dakkuri, A., and Itoh, S., Nasal absorption of ondansetron in rats: an alternative route of drug delivery. Cancer Chemother. PharmacoL, 2000, 45, 432-434. 16. Woo, Jong Soo. Nasal Absorption Studies of Granisetron in Rats Using a Validated High-performance Liquid Chromatographic Method with Mass Spectrometric Detection, Arch Pharm Res., 2006, 30(6) 778-784. 17. Results of Phase I Clinical Trial for Nasal Granisetron (US), www.snblnds.co.jp/en/release/2008/02/000051.html, last seen on December 11th, 2014. 18. Cho, H.J., Balakrishnan, P., Shim, W.S., Chung, S.J., Shim, C.K., Kim, D.D., Characterization and in vitro evaluation of freeze-dried microparticles composed of granisetron–cyclodextrin complex and carboxymethylcellulose for intranasal delivery, Int. J. Pharm., 2010, 400, 59–65. 19. Kublik H. and Muller B.W., Rheological properties of polymer solutions as carrier for nasal drug delivery systems, Eur. J. Pharm. Biopharm. 1993, 39, 192–196. 20. Jansson B., Hagerstrom H. and Fransen N., The influence of gellangum on the transfer of fluorecein dextran across rat nasal epitheliumin vivo. Eur. J. Pharm. Biopharm. 2005, 59, 557–564. 21. Souri, E., Kargar, Z., Saremi, S., Ravari, N.S., Alvandifara, F., and Amanlou, M., Development and Validation of a Stability Indicating HPLC Method for Determination of Granisetron, Journal of the Chinese Chemical Society, 2011, 58, 443-449. 22. Carlfors J., Edsman K., Petersson R. and JÖrnving K., Rheological evaluation of Gelrite in situ gels for ophthalmic use, Eur. J. of Pharm. Sci., 1998, 6, 113–119. 23. Shi-lei Cao S., Ren X., Zhang Q., Chen E., Xu F., Chen J., Liu L. and Jiang X., In situ gel based on gellan gum as new carrier for nasal administration of mometasone furoate, Int. J. of pharm. 2009, 365, 109–115.

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24. Modi, A., Tayade,. P. Enhancement of dissolution profile by solid dispersion (kneading) technique. AAPS PharmSciTech. 2006, 7(3), E87–E92. 25. Peppas, N.A. Analysis of Fickian and non-Fickian drug release from polymers. Pharm Acta Helv. 1985, 60(4),110–11. 26. Nelder, J.A., Mead, R. A simplex method for function minimization. Computer Journal. 1965, 7(4), 308–313. 27. Zuo, J., Gao, Y., Bou-Chacra, N., Löbenberg, R. Evaluation of the DDSolver Software Applications, BioMed Research International. 2014.1-9. http://dx.doi.org/10.1155/2014/204925 28. Cho, E., Gwak, H., Chun, I., Formulation and evaluation of ondansetron nasal delivery systems. Int J Pharm. 2008, 349(1-2), 101-107. 29. Moore J.W. and Flanner H.H., Mathematical Comparison of Dissolution Profiles. Pharm Technol, 1996, 20, 64-74. 30. Pires, A., Fortuna, A., Alves, G., Falcão, A., Intranasal drug delivery: how, why and what for? J. Pharm. Pharm. Sci. 2009, 12 (3), 288–311. 31. Grasdalen, H., Smidsroed, O., Gelation of gellan gum. Carbohydr. Polym. 1987, 7, 371– 393. 32. Illum, L., Nasal delivery. The use of animal models to predict performance in man. J. Drug Targeting. 1996, 3, 427–442. 33. Blum, R. A., Majumdar, A., McCrea, J., Busillo, J., Orlowski, L. H., Panebianco, D., Hesney, M., Petty, K. J., Goldberg, M. R., Murphy, M. G, Gottesdiener, K. M., Hustad, C. M., Lates, C., Kraft, W. K., Van Buren, S., Waldman, S. A., and Greenberg, H. E., Effects of aprepitant on the pharmacokinetics of ondansetron and granisetron in healthy subjects. Clin. Ther., 2003, 25, 1407-1419

Figure legend Figure 1: Rheological properties of (a) LMW alginate, (b) HMW alginate and (c) gellan gum droppable gels before and after gellation in simulated nasal fluid. Figure 2: in-vitro release profiles of granisetrone from (a) LMW alginate, (b) HMW alginate and (c) gellan gum droppable gels in simulated nasal fluid (n=3, Error bars indicate SD). Figure 3: Ex vivo permeation of granisetron HCl as a function of time from the selected droppable gels with and without enhancer through sheep nasal mucosa (n = 3). Figure 4: Histopathological sections of (a) untreated, (b) alginate gel treated, (c) gellan gum treated and (d) gellan gum /enhancer treated nasal mucosa at magnification of 100x. Granisetron is loaded in gels as 1% w/v and treatment lasted for 7h. Figure 5: (a) Mean plasma concentrations of granisetron HCl after intranasal administration of the droppable gel formula F9 (test) in comparison to the oral and IV solutions (references) to experimental animals, (b) ln-transformed data. The error bars represent ±SD.

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Table 1: Composition and evaluation of the prepared granisetron HCl droppable gels. Formula

Polymer type

F1 F2

Low molecular weight alginate

F3 F4 F5

High molecular weight alginate

F6 F7 F8 F9

Deacetylated gellan gum

Polymer conc. (%) 0.5

RE3h (%) mean±S.D Tukey confidence limits 97.89±0.4336 (96.619-98.774)

1

Farrow's constant (N) After gelling Before gelling

1.265

1.387

0.75

94.59±0.2627

(93.844-95.149)

1.189

1.321

1

92.69±0.3508

(91.792-93.535)

1.869

1.945

0.5

93.62±0.3002

(92.861-94.353)

1.326

1.567

0.75

90.46±0.3020

(89.670-91.170)

2.156

2.451

1

85.35±0.3500

(84.480-86.220)

2.786

2.870

0.1 0.2

99.31±0.2524 96.90±0.3464

(98.643-99.897) (95.839-97.561)

1.247 1.256

1.324 1.332

0.5

70.53±0.2503

(69.922-71.165)

2.769

2.984

1

Farrow's constant is calculated from the exponential formula (F N = η' G). Granisetron HCl is added as 1% in all formulae.

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Table 2: Mathematical modeling of the in-vitro release data for the selected granisetron HCl droppable gel formulae. Mathematical Model 1

Formula

Higuchi with 0

2

Korsmeyer-Peppas

2adjusted

0 (%)

KH

T90% (min)

2adjusted

n

F3

0.9203

28.455

7.141

74.282

0.9399

0.341

F6

0.9658

22.375

6.402

111.583

0.9903

0.311

F9

0.9773

22.160

5.336

161.622

0.9936

0.306

Composition of the formulae is shown in table 1. 1

Higuchi with 0 model: = 

+  √ ,

2

Korsmeyer-Peppas with 0 model:  =  

Where  is the cumulative quantity of drug released at time , 0 is burst effect and n is Korsmeyer-Peppas exponent.

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Molecular Pharmaceutics

Table 3: Ex-vivo permeation characteristics of granisetron HCl through sheep nasal mucosa.

2

Kp (cm. h-1) x10-3

Tested formulae

Jss (µg.cm-2.h-1)

mean±S.D

Tukey confidence limits

F6

208.65±5.09

69.55±3.01

(62.369-77.331)

F6+enhancer1

236.50±3.50

78.83±3.58

(69.041-86.845)

F9

444.67±5.01

148.22±3.52

(138.98-156.50)

F9+enhancer1

432.44±5.50

144.15±3.51

(135.67-153.09)

Composition of the formulae is shown in table 1. 1

2

Enhancer is 10% Hydroxypropyl β-cyclodextrin Permeation coefficient, Kp =

 

,

 = 300µg

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Table 4: Mean pharmacokinetic parameters of granisetron HCl after intranasal administration of the droppable gel formula F9 (test) in comparison to the oral and IV solutions (references) to experimental animals. Tested formula Parameter

Intranasal droppable gel 19.384±2.56

Oral solution 13.158±3.23

IV solution 31.345±2.18

AUC0-7 (µg.h/ml)

3416.155±11.38

1935.727±13.17

4718.699±12.40

AUC0-inf (µg.h/ml)

3611.731±14.12

1988.508±9.56

5523.708±15.09

0.946

0.973

0.854

90±5.52 85.56±4.18

150±7.34 57.27±0.12

------150.65±0.04

65.39%

35.99%

-------

Cmax (µg/ml)

AUC0-7/AUC0-inf Tmax (min) t1/2 (min) *Absolute bioavailability All values are mean±S.D, n=6. *Absolute bioavailability =

%&'()*+,-) /01/ %&'()*+,-) 23

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