Formulation and In Vitro Characterization of Raloxifene Nanostructured Lipid Carriers For Oral Delivery With Full Factorial Design-Based Studies Using Quality By Design (QbD) Approach

The main aim of the present study is to improve the dissolution rate of Raloxifene Hydrochloride by formulating nanostructured lipid carriers (NLC) using Quality by Design (QbD) approach. The formulations of NLC-RH were prepared by the ultrasonication method using stearic acid as solid lipid, medium-chain triglyceride as the liquid lipid and polysorbate 80 as the surface-active agent. Two most critical quality attributes (CQAs) for NLC-RH were particle size and entrapment efficiency. The other attributes of medium influence identified includes dissolution rate, zeta potential and particle size didtribution. The Critical Material Attributes (CMAs) identified were solid lipid/liquid lipid ratio and surfactant concentration. The time required for ultrasonication was selected as a Critical Process Parameter (CPP). The 23 full factorial design was used to evaluate the relationship between the CMAs and CPPs variable. Based on the experiments, the composition of the optimal formulation is achieved with solid lipid/liquid lipid ratio of 7:3 and 7 % of surfactant concentration with 15 min of ultrasonication time. The optimized formulation of NLC-RH was found to be with a mean particle size of 146 nm with narrow particle size distributions. From the above results, it is concluded that a promising Raloxifene HCl loaded NLC could give a novel and potential therapy for osteoporosis.

cle size and entrapment ef iciency. The other attributes of medium in luence identi ied includes dissolution rate, zeta potential and particle size didtribution. The Critical Material Attributes (CMAs) identi ied were solid lipid/liquid lipid ratio and surfactant concentration. The time required for ultrasonication was selected as a Critical Process Parameter (CPP). The 2 3 full factorial design was used to evaluate the relationship between the CMAs and CPPs variable. Based on the experiments, the composition of the optimal formulation is achieved with solid lipid/liquid lipid ratio of 7:3 and 7 % of surfactant concentration with 15 min of ultrasonication time. The optimized formulation of NLC-RH was found to be with a mean particle size of 146 nm with narrow particle size distributions. From the above results, it is concluded that a promising Raloxifene HCl loaded NLC could give a novel and potential therapy for osteoporosis.

INTRODUCTION
Osteoporosis(OP) is a disorder of bone elements and their quality (Lorentzon and Cummings, 2015). Out of many causes for OP, the most important is postmenopausal osteoporosis and is considered as high risk for women (Sozen et al., 2017). About 30-40 % of women are estimated to suffer from this disorder (Curtis and Safford, 2012).
Pharmacological measures for treating postmenopausal osteoporosis include use of drugs like activated vitamin D3, Calcitonin, Biphosphonates, Hormone Replacement Therapy (HRT) with Estrogen, Anabolic steroids, Calcium supplements and use of selective estrogen receptor modulators (Brar, 2010). Though HRT is an effective treatment of postmenopausal osteoporosis, complications like deep vein thrombosis and occurrence of endometrial and breast cancer make it less preferred as the irst line of therapy (Gambacciani and Levancini, 2014). Raloxifene, a second-generation Benzothiopene derivative that is prescribed for treatment and prevention of osteoporosis (Maximov et al., 2013).
Raloxifene, marketed as a Raloxifene Hydrochloride compound approved for the prevention and treatment of PMO fractures. It has signi icantly less solubility and very low bioavailability (of less than 2 %) with inter-subject variability. Raloxifene undergoes external hepatocellular metabolism in the liver.
The NLCs are formulated with combination of solid lipid with liquid lipid, which improved the encapsulation of drug and prevents drug expulsion during storage. Moreover, NLC formulations have the advantages of prolonged drug release, biocompatibility and easy of scaling-up its production (Mukherjee et al., 2009;Mohammadi-Samani and Ghasemiyeh, 2018). The in vivo digestion (by lipases and co-lipases) of NLCs, once reaching the small intestine, converts them into mixed micelles that are ready for drug absorption (Elmowafy et al., 2017). The objective of the present study was to explore the feasibility to encapsulate Raloxifene Hydrochloride into NLCs to improve the dissolution rate and eventually oral bioavailability. The NLC formulation has the advantages for prolonged drug release with improved bioavailability and easy for production. The improved bioavailability is due to its encapsulation of drug with lipid carriers.

Materials
Raloxifene Hydrochloride was used as the drug candidate. Stearic acid (Stelliesters Glycerol) and MCT (Stelliesters MCT 65/35) were evaluated as the solid lipid and liquid lipid, respectively. Polysorbate 80 (Tween 80) and Lecithin were explored as the hydrophilic and lipophilic surfactants. Silicon Dioxide (Syloid XDP 3150) was used as the adsorbent. The compounds mentioned above were received as gift samples from Cadila Pharmaceuticals Ltd., Ahmedabad.

De ining QTPP
QbD based approach is to de ine the quality target product pro ile (QTPP) based on product requirement and intended performance. Target product pro ile (TPP) includes route of administration, maximum and minimum doses, and appearance is better appropriate quality, safety and ef iciency features of drug product such as stability, pharmacokinetic properties, bioavailability, purity, drug release proile etc. depending on the speci ic dosage form and therapeutic properties.

Determination of CQAs
The CQAs are the critical attributes of the products which ensure the consistency in the product performance. The CQAs are derived from QTPP and are based on prior product knowledge and process understanding. CQAs include the physical, chemical, biological and microbiological attributes that are within an appropriate limit, range or distribution to ensure the desired product quality. The CQAs may include particle/droplet size, entrapment ef iciency, zeta potential, poly dispersibility index (PDI), drug release as shown in Table 1.

Determination of the CMAs and CPPs
The QbD determine the material attributes and process parameters based on experimental conditions and also relationships between these material attributes and process parameters to the drug product CQAs. Factors are considered based on properties of API and excipients used in the preparation of NLCs and from process parameters (ultrasonication time and temperatures) as shown in Table 2.

Drug polymer interaction study
To verify the purity of the obtained samples like drug and excipients, the obtained FTIR spectra were veri ied (FTIR BRUKER) over a wavelength range of 4000-400cm −1 at resolutions of 4cm −1 sample were directly placed on the probe and spectra were recorded.            The FTIR spectra of pure Raloxifene Hydrochloride and mixture of all the ingredients used in preparations of NLCs were observed to ind any interactions between the drug and excipients.

Construction of calibration curve of RH
For spectral scanning, 100 mg of RH drug was readily dissolved in 100 ml of a suitable solvent. One ml of prepared stock solution was further diluted to 100 ml with the same solvent (10 µg/ml) and inally scanned for maximum absorbance using UV spectrophotometer (UV-1800 SHIMADZU) in the range from 200 to 400 nm, maximum absorbance was found at 286 nm was 0.998, for methanol as a solvent, the standard graph of RH in Methanol has also shown a line of good it over a concentration range of 0 to 10 µg/ml.
The drug was analyzed spectrophotometrically at 286 nm, with an R 2 value of 0.998.

Preparation of NLC-RH
The Raloxifene Hydrochloride (RH) loaded NLCs were formulated by using high-speed homogenization followed by ultrasonication. The lipid and aqueous phases were prepared separately. Lipid phase consists of solid lipid (stearic acid), liquid lipid (MCT 55/45) and 0.5% lecithin as the lipophilic emulsi ier, while the aqueous phase consisted of hydrophilic emulsi ier (Tween 80) dissolved in distilled water. RH was dissolved in MCT and then mixed with other lipid phase components. All components of the lipid phase were heated separately to 10 • C above solid lipid transition temperatures for 10 min before mixing. The aqueous phase was added drop-wise to the molten lipid phase and mixed using a high-speed homogenizer (Janke & Kunkel, GmbH, Staufen, Germany) at 10,000 rpm for 10 min. The mixture was further treated using a probe-type sonicator (ultrasonic processor, GE130, probe CV18, Newtown, CT). The resultant emulsions were adsorbed on to the granular colloidal silicon dioxide and cooled at room temperature. The NLC adsorbed powder was compressed into tablets.

Formulation Optimization of RH-NLC as per Design of Experiments (DoE)
The formulation that meets the desired CQAs is the ultimate goal of all formulation development activities. The formulation components of NLC-RH that have a high potential to impact the drug product CQAs are the ratio of solid lipid/liquid lipid ratio, the surfactant concentration (polysorbate 80) and the ultrasonication time as shown in Table 3. The water quantity, the temperature has a low to medium risk to impact the CQAs. As Raloxifene Hydrochloride is a nanoparticulate formulation, particle size is the most critical quality attributes to study. In addition to this, the encapsulation ef iciency (%) of the Raloxifene HCl in nanostructured lipid particles is also considered as the dependent variable.
Therefore, particle size (PS) and % entrapment ef iciency (% EE) was selected as an output response. Hence, to achieve optimum performance, the formulation design space has to be established within which all the CQAs are met.
To achieve this, a 2 3 full factorial design with three centre point study was used to optimize the levels of solid/liquid lipid ratio, Surfactant concentration and ultrasonication time to establish the formulation and process space.
Statistical design and analysis were conducted using the software Design Expert 7.0. (trial version). The trials were conducted randomly in the order given by the software to avoid any intentional error. An overview of different formulations is done by changing the ratio of solid/liquid lipids, surfactant concentration and ultrasonication time is shown in below Table 4.

Statistical Analysis
A full factorial design was used to study the dependence between the formulation variables (independent variables: X 1 , X 2 , X 3 ) and dependent variables (Malvey et al., 2020) (Responses: Y 1 , Y 2 ) the following generation of the polynomial equation from software and experimental values are incorporated into it, as shown in Table 5.
Where Y represents the overall predicted response (Particle size, entrapment ef iciency) β 0 is the overall intercept, β 1 β 2 β 3 are individual intercept of the main effect of X 1 , X 2 , X 3 . The ANOVA studies are generated from the software to evaluate the p-values, Fratio, and lack of it. To evaluate the itting extent of the experimental data regression coef icient (R 2) and adjusted R 2 were determined. 3D and counterplots prediction was made to run further experimental studies for estimation of model accuracy.

Particle size analysis
The particle size was determined by laser particle size analyzer (Zetatrac 10.6.2, Microtrac Inc.) using the distilled water as a dispersant. The dispersed nanoparticle was added to the sample dispersion unit containing stirrer. The average particle size was measured after experimenting triplicate.

Zeta potential
The prepared NLC were carried out for Zeta potential estimation by using binocular microscopy (Model CH20iBIMF), particle size was recorded by calibrations of stage micrometre division and eyepiece micrometre division. Further particle analysis was carried out by using Zeta sizer (Malvern, Model: Nano ZS90). The Average size of NLCs was expressed in d. nm, and a charge is measured.

Drug encapsulation ef iciency (%)
Drug encapsulation ef iciency (EE) was conducted through an indirect method where an aliquot (2 ml) of RH-loaded NLCs was centrifuged at 100,000 RPM for 2h at 4 0 C using a Beckman Optima T M Ultracentrifuge (Optima T M XL, Indianapolis, IN). The proportion of free drug (RH) supernatant luid was measured spectrophotometrically (Shimadzu, the model UV-1800 PC, Kyoto, Japan) at 286 nm against the blank. The following equation then calculated the encapsulation ef iciency: Where EE % is the percentage of encapsulation ef iciency, Da is the amount of drug added during preparation of NLCs and Df is the amount of free drug present in the supernatant luid after centrifugation.

Surface morphology study (SEM)
Scanning electron microscopy (Zeiss, TIFR, Mumbai) of an optimized formulation of NLC-RH was evaluated to ind the particle size and surface topography.
The photographs were taken using an SEM under magni ication of 10 KX-12 KX.

In vitro drug release
In vitro diffusion studies were carried out by using two open-ended dialysis tubes with an arti icial membrane using an optimized formulation of NLC-RH. The prepared Raloxifene Hydrochloride NLCs were re-dispersed in 5 ml of USFDA's OGD (Of ice of Generic Drugs) recommended media, i.e., 0.1% polysorbate 80 in puri ied water and subjected to dialysis by immersing the dialysis tube to the receptor compartment containing 50 ml of 0.1% polysorbate 80 in water. The receptor medium was agitated continuously using a magnetic bead under magnetic stirrer, and the temperature was maintained at 37 ± 0.5 • C. 0.5 ml sample of receptor compartment was taken at predetermined time intervals for 1 hr and each time replaced with 0.5 ml of fresh media. The amount of drug released was determined spectrophotometrically at 286 nm.

Differential scanning calorimetry (DSC)
It is based on the principle of measurement of heat low in and out of sample and reference for the period of the controlled temperature cycle, merely 5-10 mg sample was sealed in aluminium pan followed by heating at the rate the of 20 • C/min over the temperature range of 10-200 • C under liquid nitrogen low rate 40 ml/min and thermogram was obtained. The thermal behaviours of pure drug substance are applied.

RESULTS AND DISCUSSION
The purpose of this study was to develop lipid-based NLCs of raloxifene hydrochloride for the treatment of osteoporosis. NLC-RH was prepared by emulsiication using high-speed homogenization followed by ultrasonication. A 2 3 full factorial design with three centre point was employed.

Drug polymer interaction study
Fourier transform infrared spectroscopic (FTIR) analysis was used to identify any interaction between the molecules used in the preparation of formulation. The FTIR studies show that there are no interactions between the molecules and the preparations of NLCs, as shown in Figure 1 and Figure 2, corresponding values are plotted in Table 6.

Results of DSC
As DSC thermogram is shown in Figure 3, piercing endothermic peak at 278.48 • C was observed in the inalized formulation, corresponding to melting point observed in DSC of Pure drug was 289.88 • C as shown in Figure 3, but the slight difference to pure form of the drug in the image view.

SEM (Scanning Electron Microscopy)
The NLCs are observed under scanning electron microscopy. A topographical characterizing technique shows detailed surface examination at the molecular level. The optimized formulation is represented in Figure 4.

Particle Size (PS) and Zeta Potential
The prepared NLC-RH showed particle size between 278.2 and 648.6 nm. The average diameter and zeta potential of optimized formulation were determined by photon correlation spectroscopy (PCS) at room temperature. The average particle size of optimized formulation was in the range of 278.2 nm with a maximum intensity of 536.0 nm particles. It shows the broader range of particle size distribution from 1635 nm to 72.30 nm. The value greater than +25 mV or less than -25 mV has a high degree of stability. Zeta potential was found to be 0.52 mV for optimized formulation. Thus it suggests that possible aggregation of particles as shown in Figure 5 along with values. The inal equation was generated in the coded form by the software was given below from 3D graphs, as shown in Figure 6.
The F-value of 448.63 implies the model is signi icant; the p-value is less than 0.0500 indicate model terms are signi icant. In this case, AC, ABC are significant model terms. The remaining model terms are not signi icant due to its values greater than 0.05.  : 3D images of contour plots for particle size equation was generated in the coded form by the software was given below 3D graphs, as shown in Figure 7.

In-vitro drug release studies
In-vitro release studies were performed in 0.1% polysorbate 80 in puri ied water. A slow release of Raloxifene up to 12 hrs was observed. DSC results indicated that the Raloxifene entrapped in the NLCs. The Scanning electron microscope (SEM) has revealed that the NLCs are obtained as a spherical-shaped carrier system.
The highest correlation coef icients were obtained for the Korsmeyer-Peppas model, to follow Non-Fickian diffusion for the drug release, as shown in Table 7.
The results demonstrated that raloxifene hydrochloride NLCs with such ingredients could be an emerging delivery method for the long-term treatment of osteoporosis.

Marketed Formulation
The obtained dissolution graph of NLCs is com- parted with the marketed formulation and found to be sustained release of medication without sudden increased in concentration, as shown in Figure 8.

Statistical Analysis
The experiments results were determined by the half-normal plot and Pareto chart to ind signi icant effects of X 1 X 2 X 3 variables. The higher tvalues observed in the pereto chart was for particle size and entrapment ef iciency, as shown in Figure 9. The results indicate that the concentration of solid/liquid lipid ratio and surfactant exhibits the highest effect in altering the particle size and encapsulation ef iciency as compared to the time required for sonication. The experimental data were analyzed and itted to various models (liner, interactive and quadratic) the results showed the liner order model exhibited highest regression R 2 hence linear model was adopted to it the experimental data and to ind an interaction between formulation variable and dependent variables.
ANOVA analysis depicted that developed linear model was highly signi icant with low P-value which is less than 0.05 with the well it was checked by R 2 value for particle size and entrapment ef iciency (0.9984), (0.9986).
Further, more, a high degree precision of experiment was indicated by low values of coef icient of variation CV= 2.38% the adequate precession measures signal to noise ratio, and a ratio greater than four is desirable to navigate design space for the constrain selected as shown in Table 9, An Studentized residual versus the experimental run and residual versus run was constructed to ensure the obtained data.
The relationship between encapsulation ef iciency and formulation variable model graphs, mainly 3D graphs and contour plots were generated to assess the individual ad interactive effect on the response.

Optimization and validation
Regression model developed in the study is to found optimum formulation with the desired value from 3D graphs. A coded value was found to X 1 =+1, X 2 = -0.2, X 3 = 0 the corresponding experimental parameters for X 1 =7:3, X 2 = 7%, X 3 = 15 minutes, were respectively under the optimum condition the experimental predicted particle size was 150 nm as shown in Table 8.
However, considering the optimum condition for X 2 can be modi ied as the coded value of +1 that is 7.5 % of surfactant concentration, the statistical conclusion was given for the model to prove the model is the best it, as shown in igure 9.
To compare the predicted results with experimental values additional data experiment was performed in triplicate under the new experimental condition the particle size found to be 146 microns and well-matched with the predicted response of 150 microns, the percentage error was found to be -2.67 which, is less than 5 % and it falls in an acceptable limit.
Likewise, for encapsulation ef iciency the experimental value found to be 89% and well-matched with predicted response 86%, the percentage error was found to be +3.488 which is less than 5 %, and it falls in the acceptable limit, as shown in Table 10.

CONCLUSION
The present research paper establishes a successfully optimized composition of nanostructured lipid carriers of raloxifene hydrochloride, designed by QbD approach and optimized by DoE tool. The optimized composition was derived from the initial risk assessment, preformulation studies and using the design of experiment (DoE) concept. The initial risk assessment was carried out to identify the critical formulation variables (CFVs) and critical process parameters (CPPs) that have a most likely impact on the critical quality attributes (CQAs). Based on the initial risk assessment, two CQAs, namely particle size and percentage entrapment ef iciency, were found to be the most critical attributes for the NLC-RH. Besides, the CQAs that are found to be of medium impact are Zeta potential and Dissolution rate. The CFVs found to be the solid lipid/liquid lipid ratio and surfactant concentration and the most critical CPP found to be the ultrasonication time. The 2 3 full factorial design studied the impact of CFVs and CPP on the CQAs of the drug product with three centre points. The optimized composition of NLC-RH was found to be with solid to liquid lipid ration of 7:3, with 7 % surfactant concentration and 15 minutes of ultrasonication time. Future development of NLC-RH would be facilitated by an in-vivo performance with enhanced practical understanding. Based on these above results, it can be concluded that a promising Raloxifene HCl loaded NLC could be developed, which can be a potential alternative therapy for osteoarthritis for extended period of time compared to conventional preperation.

ACKNOWLEDGMENT
The author is thankful to lead guide and co-guide for their continuous support, for their support in developing this article.