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International Journal of Healthcare and Medical Sciences
ISSN(e): 2414-2999, ISSN(p): 2415-5233
Vol. 4, Issue. 6, pp: 117-122, 2018
URL: http://arpgweb.com/?ic=journal&journal=13&info=aims
Academic Research Publishing
Group
*Corresponding Author
117
Original Research Open Access
Formulation and Evaluation of Polymeric Nanoparticles of Rifampicin for Anti-
Tubercular Therapy
Dr. Sameer S. Sheaikh*
Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India
Shrikrishna K. Harkal
Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India
Rahul P. Gaikwad
Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India
Rahul W. Gawali
Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India
Dinesh P. Deshmukh
Uttamrao Deshmukh Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India
Abstract
Polymeric Nanoparticles of Rifampicin were prepared by emulsion solvent evaporation technique using poly methyl
methacrylate as polymer matrix and Poly vinyl alcohol as surfactant. Drug entrapped free flowing nanoparticles of
Rifampicin were obtained after optimization using 32 factorial design and characterized for entrapment efficiency,
particle size distribution, differential scanning calorimetry (DSC), X-ray diffraction (XRD), scanning electron
microscopy (SEM) and in vitro and stability studies. The PMMA nanoparticles had a small size (213 ± 0.72 nm),
uniform size distribution. The effects of dependent variables drug-polymer ratio and surfactant concentration on
particle size and encapsulation efficiency were studied. The drug and polymer were not interacting with each other.
SEM studies revealed the spherical shape of nanoparticles and in vitro release studies showed sustained drug release.
RIF-polymeric nanoparticles drug delivery system proved to be promising for anti-tubercular therapy.
Keywords: Rifampicin; Polymeric nanoaprticles; Poly methyl methacrylate; Particle size.
CC BY: Creative Commons Attribution License 4.0
1. Introduction
Tuberculosis is a chronic infectious disease caused by the infection of Mycobacterium tuberculosis, which is the
foremost cause of death worldwide and its incidence is increasing particularly in association with AIDS pandemic.
Now a days multiple drug chemotherapy forms the backbone of antituberculotic therapy. Particularly, rifampicin is
the first choice drug in the treatment of tuberculosis. But the current treatment of tuberculosis involves prolonged
oral administration of large systemic doses of combined antibiotics, which are associated with unwanted side effects
and poor patient compliance [1]. The polymeric nanoparticles (PNPs) are prepared from biocompatible and
biodegradable polymers where the drug is dissolved, entrapped, encapsulated or attached to a nanoparticle matrix.
PNPs are promising vehicles for drug delivery by easy manipulation to prepare carriers with the objective of
delivering the drugs to specific target, such an advantage improves the drug safety. Polymer-based nanoparticles
effectively carry drugs, proteins, and DNA to target cells and organs [2].
Even though the development history of polymeric nanoparticles-based antimicrobial drug delivery systems is
relatively shorter than other nanoparticle systems such as liposomes and SLNs. Nanoparticles have shown great
therapeutic potentials.
1.1. Advantages of Polymeric Nanoparticles [3, 4]
• Increases the stability of any volatile pharmaceutical agents, easily and cheaply fabricated in large quantities
by a multitude of methods.
• They offer a significant improvement over traditional oral and intravenous methods of administration in terms
of efficiency and effectiveness.
• Delivers a higher concentration of pharmaceutical agent to a desired location.
• The choice of polymer and the ability to modify drug release from polymeric nanoparticles have made them
ideal candidates for cancer therapy, delivery of vaccines, contraceptives and delivery of targeted antibiotics.
• Polymeric nanoparticles can be easily incorporated into other activities related to drug delivery, such as tissue
engineering.
International Journal of Healthcare and Medical Sciences
118
In the present study, we examined the potential of polymeric nanoparticles for oral anti-tubercular drug delivery.
The aim of our study was to formulate nanoparticles incorporating the lipophilic drug Rifampicin and evaluate its
release and absorption from these in vitro.
2. Materials & Methods
2.1. Materials
Rifampicin was obtained as a gift sample from Lupin Pharma Pvt. Ltd. Aurangabad. Polu methyl methacrylate
was received as a gift sample from Prachi Enterprises Pvt. Ltd., Mumbai. Poly vinyl alcohol was a gift sample from
BASF, Mumbai. All other chemicals and reagents were of analytical grade and were used without further
purification.
2.2. Methods
2.2.1. Preparation of RIF- Nanoparticles
Polymeric Nanoparticles were prepared by Emulsion solvent evaporation method. Required quantity of polymer
and drug were weighed & dissolved in 12ml of dichloromethane. Quantity of PVA was mixed with 30ml of water &
this solution was kept in another beaker.Both the phases were kept for sonication for 15 min. until it become clear.
Solution containing drug and polymer were added drop wise to aqueous phase under continues stirring. The formed
nanoparticles suspension were homogenized at 18000 rpm for 15min then followed by magnetic stirring for 3hr. The
suspension was centrifuged at 9,000 rpm. for 45 min. The samples were added to glass vials & freeze-dried with
mannitol 2% (w/v) as cryprotectant in a lyophilizer.
2.2.2. Total Drug Content (TDC) and Entrapment Efficiency (EE)
The total amount of drug per unit volume was determined by suitably disrupting 1ml of the dispersion in 10ml
suitable solvent volumetrically. Total drug content was determined by using the equation given below:
EE was determined by analyzing the clear supernatant obtained by centrifuging the developed SLN dispersions
using Remi Ultracentrifuge. The EE was calculated as follows:
Where Df = Amount of drug in clear supernatant fluid.
2.2.3. Particle Size Analysis
Nanoparticles formulation was characterized for particle size using Malvern 2000. Double distilled water was
used as a dispersant medium.
2.2.4. Particle Shape and Surface Morphology
Scanning Electron Microscopy (SEM) analysis of the prepared nanoaprticles was carried out to study the
morphology like sphericity and aggregation. Sample was examined by SEM (Jeol, JSM-6360).
2.2.5. FT-IR Spectroscopy
Drug was characterized by FT-IR spectroscopy. The spectrum was recorded using FT-IR spectrophotometer
(Jasco, FT/IR-4100). The scanning range was 4000 to 400cm-1
. The spectrum of RIF is shown in Figure No. 2. The
samples were previously dried and mixed thoroughly with Potassium bromide in 1:5 (Sample:KBr) were obtained at
a resolution of 2 cm-1
from 4000 to 400 cm-1
.
2.2.6. Differential Scanning Calorimetry (DSC)
DSC measurements were performed on differential scanning equipped with an intra-cooler (DSC Mettler STAR
SW 9.01). Inert atmosphere was maintained by purging Nitrogen gas at a flow rate of 50ml/min. RIF and RIF-
Nanoparticles, approximately 3-5mg of each sample was heated in aluminium pan from 40 0
C to 240 0
C at heating
rate of 10 0
C/min under a stream of Nitrogen at flow rate of 20ml/min.
2.2.7. X-Ray Diffraction (XRD) Study
X-Ray diffraction patterns of the powdered samples of the drug RIF and carrier were recorded using Philips
PW3710 Analytical XRD B.V. X-Ray diffractometer using CU K 2α-rays with a voltage of 40kV and a current of
25mA. Samples were scanned for 2θ from 5 to 500
C. Diffraction pattern for RIF was obtained.
2.2.8. In vitro Drug Release Study
Rifampicin loaded nanoparticles formulation equivalent to drug dose (250 mg) was filled in (size“0”) capsule.
The quantitative in vitro release test was performed in two different GI environment i.e. 0.1N HCl (stomach), 6.8 pH
buffer. At first two hours, in vitro release test was performed in 900 mL (0.1N HCl). This study was then continued
for four hours in 900 ml (6.8 pH buffer solution) maintained at 37 ± 0.5°C using USP type I dissolution apparatus.
The basket were rotated at 50 rpm. 5 ml aliquots was collected periodically (30, 60, 90, 120, 150, 180, 210, 240, 270,
300, 330, 360, 390, 420, 450, 480) and replaced with fresh dissolution medium. Aliquots, after filtration through
whatman filter paper #45 and diluted . Analysis was carried out using UV spectrophotometer. Results were
compared with pure rifampicin. The dissolution experiments were carried out in triplicate, and data were expressed
as mean ± S.D.
International Journal of Healthcare and Medical Sciences
119
2.2.9. Anti-Microbial Study
The antimicrobial study of formulated rifampicin nanoparticles was carried out by using agar gel diffusion
method. In which weighed 9 gm of Agar-Agar and 5 gm of nutrient broth mixed it into 300 ml of DW. The prepared
nutrient medium placed in Autoclave and start sterilization cycle according to IP 2007, in which holding time
becomes 30 min to 60 min at 15 psi pressure and temperature reaches up to 1150
C to 1380
C after completion of
cycle, nutrient medium was transferred into sterile petri-plates for cooling. Cultured microorganism Bacilus subtilis
(B. subtilis), Staphylococcus aureus (S. aureus) etc. were spread on nutrient medium then the prepared suspension of
nanoparticles and pure drug were poured into the well and kept it into the freeze for 20 min. then petriplates were
incubated for 12 hrs and finally observed the plates for calculating zone of inhibition.
3. Result & Discussion
3.1. Characterization of RIF-Polymeric Nanoparticles
Nanoparticles were prepared using poly methyl methacrylate and Poly vinyl alcohol (Surfactant). The
Nanoparticles formulation exhibited a small particle size below 213nm and a TDC of >95% (w/v) with Entrapment
efficiency 96.04%.
Table-1. Experimental runs with results of response
Batch
X1
polymer
(mg)
X2
Surfactant
(%)
Drug
(mg)
Y1
Entrapment
Efficiency (%)
Y2
Particle size
(nm)
F1 750 1.5 100 91.08 ± 0.23 723 ± 0.43
F2 1000 2.5 100 78.95 ± 0.48 831 ± 0.82
F3 750 2 100 89.82 ± 0.82 527 ± 0.29
F4 1000 2 100 76.8 ± 0.56 713 ± 0.81
F5 500 2.5 100 89.43 ± 0.21 384 ± 1.03
F6 500 2 100 90.67 ± 1.04 324± 0.89
F7 500 1.5 100 92.04 ± 0.63 540 ± 0.39
F8 750 2.5 100 96.04 ± 1.03 213 ± 0.72
F9 1000 1.5 100 80.12 ± 0.87 921 ± 0.41
3.2. Particle Shape and Surface Morphology
The morphology of nanoparticles is similar as they appear generally well formed and characterized by a
spherical shape. Shown in Figure No. 1 (A) below:
Figure-1. (A) SEM of Optimized Formulation F-8, (B) Particle size distribution for Optimized Formulation F-8
3.3. Particle Size
The mean particle size of the RIF-Nanoparticles formulation was 213nm showed in Figure No. 1 (B).
3.4. Infrared Spectroscopy
IR spectra of pure drug RIF and formulation showed no interaction with the drug and prominent peaks of the
drug were not affected. Hence drug-excipients compatibility was established suggesting that there is no interaction
between RIF and other excipients or no degradation of drug molecule.
International Journal of Healthcare and Medical Sciences
120
Figure-2. FTIR Spectrums of (A) Pure drug RIF, (B) Formulation batch F8
3.5. Differential Scanning Calorimetry
DSC of RIF observed has been shown in Figure No. 3.
Figure-3. Overlay of DSC curve of Drug and Formulation
DSC curve presents an endothermic peak with Tonset at 174.200
C, Tp (temperature of peak) at 191.740
C and Tf
(temperature of extrapolated end set) at 198.600
C. The sharp endothermic peak Tp at 191.740
C (actual M.P. 1860
C)
corresponds to the melting point of RIF which confirms with value mentioned in the literature.
3.6. X-Ray Diffraction Study
As XRD was performed to confirm the findings obtained by DSC, the X-ray patterns of Rifampicin and RIF-
Nanoparticles are shown in Figure No. 4.
International Journal of Healthcare and Medical Sciences
121
Figure- 4. X-ray Diffraction Patterns of (A) Pure Drug RIF,(B) Optimized Formulation F-8
3.7. In vitro Drug Release Study
The in vitro drug release of F8 formulations is shown in Figure No. 5.
Figure-5. (A) in vitro drug release profile comparison (B) In vitro drug release graph for F-1 to F-9
From Figure No. 5, In vitro drug releases from formulation F-1 to F-9 were carried out. From the above drug
release study it is found that formulation F-8 showed better drug release (90.48%) in 8hrs compared to others.
3.8. Anti-Microbial Study
Antimicrobial activity of RIF-Nanoparticles was carried out with the individual component by using agar gel
diffusion method. In that method Bacilus subtilis (B. subtilis), Staphylococcus aureus (S. aureus) cultured
microorganisms were used. From the Figure No. 6, the zone of inhibition of each component was observed, in that
zone of inhibition of formulation and the pure drug were clearly observed. The above observation might be
concluded that the RIF-Nanoparticles had great antimicrobial potential which may further apply for various medical
applications.
International Journal of Healthcare and Medical Sciences
122
Figure-6. Antimicrobial activity of RIF-Nanoparticles on microorganism (A) B. subtilis, (B) S. aureus
(A) (B)
Table-2. Observation Table for Microbial Assay
Microorganism
Diameter
Plain Drug Formulation
Staphylococcus aureus
3.2 ± 0.05cm 3.5 ±0.23 cm
3.3 ± 0.15cm 3.6 ±0.057 cm
3.2 ± 0.057cm 3.6 ± 0.20 cm
Bacilus subtilis
2.5 ± 0.15cm 2.9 ± 0.15cm
2.1 ±0.15cm 2.7 ± 0.208cm
2.2 ± 0.15cm 2.3 ± 0.15cm
4. Conclusion
In the present study, polymeric nanoparticles of Rifampicin were developed to a satisfactory level in terms of
particle size, drug entrapment, drug release and antimicrobial activity. The particles were found to be spherical and
smooth. The drug release data shows satisfactory results when compared with drug and marketed formulation. The
antimicrobial study shows good zone of inhibition when compared with plain drug. So these drug delivery systems
have potential to treat tuberculosis.
References
[1] Vyas, S. P., Kannan, M. E., Jain, S., Mishra, V., and Singh, P., 2004. "Design of liposomal aerosols for
improved delivery of rifampicin to alveolar macrophages." Int. J. Pharm, vol. 269, pp. 37–49.
[2] Shokri, N., Akbari, J. H., Fouladdel, S. H., Khalaj, A., Khoshayand, M. R., and Dinarvand, R., 2011.
"Preparation and evaluation of poly (caprolactone fumurate) nanoparticles containing Doxorubicin HCL."
DARU, vol. 19, pp: 12-22
[3] Abhilash, M., 2010. "Potential applications of Nanoparticles." Int J Pharm Bio Sci., vol. 1, pp: 1-12
[4] Kayser, O. A. L. and Hernández-Trejo, N., 2005. "The Impact of nanobiotechnology on the development of
new drug delivery systems." Current Pharmaceutical Biotechnology, vol. 6, p. 35.

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Formulation and Evaluation of Polymeric Nanoparticles of Rifampicin for Anti-Tubercular Therapy PDF

  • 1. International Journal of Healthcare and Medical Sciences ISSN(e): 2414-2999, ISSN(p): 2415-5233 Vol. 4, Issue. 6, pp: 117-122, 2018 URL: http://arpgweb.com/?ic=journal&journal=13&info=aims Academic Research Publishing Group *Corresponding Author 117 Original Research Open Access Formulation and Evaluation of Polymeric Nanoparticles of Rifampicin for Anti- Tubercular Therapy Dr. Sameer S. Sheaikh* Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India Shrikrishna K. Harkal Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India Rahul P. Gaikwad Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India Rahul W. Gawali Durgamata Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India Dinesh P. Deshmukh Uttamrao Deshmukh Institute of Pharmacy, Dharmapuri, Parbhani Maharashtra, India Abstract Polymeric Nanoparticles of Rifampicin were prepared by emulsion solvent evaporation technique using poly methyl methacrylate as polymer matrix and Poly vinyl alcohol as surfactant. Drug entrapped free flowing nanoparticles of Rifampicin were obtained after optimization using 32 factorial design and characterized for entrapment efficiency, particle size distribution, differential scanning calorimetry (DSC), X-ray diffraction (XRD), scanning electron microscopy (SEM) and in vitro and stability studies. The PMMA nanoparticles had a small size (213 ± 0.72 nm), uniform size distribution. The effects of dependent variables drug-polymer ratio and surfactant concentration on particle size and encapsulation efficiency were studied. The drug and polymer were not interacting with each other. SEM studies revealed the spherical shape of nanoparticles and in vitro release studies showed sustained drug release. RIF-polymeric nanoparticles drug delivery system proved to be promising for anti-tubercular therapy. Keywords: Rifampicin; Polymeric nanoaprticles; Poly methyl methacrylate; Particle size. CC BY: Creative Commons Attribution License 4.0 1. Introduction Tuberculosis is a chronic infectious disease caused by the infection of Mycobacterium tuberculosis, which is the foremost cause of death worldwide and its incidence is increasing particularly in association with AIDS pandemic. Now a days multiple drug chemotherapy forms the backbone of antituberculotic therapy. Particularly, rifampicin is the first choice drug in the treatment of tuberculosis. But the current treatment of tuberculosis involves prolonged oral administration of large systemic doses of combined antibiotics, which are associated with unwanted side effects and poor patient compliance [1]. The polymeric nanoparticles (PNPs) are prepared from biocompatible and biodegradable polymers where the drug is dissolved, entrapped, encapsulated or attached to a nanoparticle matrix. PNPs are promising vehicles for drug delivery by easy manipulation to prepare carriers with the objective of delivering the drugs to specific target, such an advantage improves the drug safety. Polymer-based nanoparticles effectively carry drugs, proteins, and DNA to target cells and organs [2]. Even though the development history of polymeric nanoparticles-based antimicrobial drug delivery systems is relatively shorter than other nanoparticle systems such as liposomes and SLNs. Nanoparticles have shown great therapeutic potentials. 1.1. Advantages of Polymeric Nanoparticles [3, 4] • Increases the stability of any volatile pharmaceutical agents, easily and cheaply fabricated in large quantities by a multitude of methods. • They offer a significant improvement over traditional oral and intravenous methods of administration in terms of efficiency and effectiveness. • Delivers a higher concentration of pharmaceutical agent to a desired location. • The choice of polymer and the ability to modify drug release from polymeric nanoparticles have made them ideal candidates for cancer therapy, delivery of vaccines, contraceptives and delivery of targeted antibiotics. • Polymeric nanoparticles can be easily incorporated into other activities related to drug delivery, such as tissue engineering.
  • 2. International Journal of Healthcare and Medical Sciences 118 In the present study, we examined the potential of polymeric nanoparticles for oral anti-tubercular drug delivery. The aim of our study was to formulate nanoparticles incorporating the lipophilic drug Rifampicin and evaluate its release and absorption from these in vitro. 2. Materials & Methods 2.1. Materials Rifampicin was obtained as a gift sample from Lupin Pharma Pvt. Ltd. Aurangabad. Polu methyl methacrylate was received as a gift sample from Prachi Enterprises Pvt. Ltd., Mumbai. Poly vinyl alcohol was a gift sample from BASF, Mumbai. All other chemicals and reagents were of analytical grade and were used without further purification. 2.2. Methods 2.2.1. Preparation of RIF- Nanoparticles Polymeric Nanoparticles were prepared by Emulsion solvent evaporation method. Required quantity of polymer and drug were weighed & dissolved in 12ml of dichloromethane. Quantity of PVA was mixed with 30ml of water & this solution was kept in another beaker.Both the phases were kept for sonication for 15 min. until it become clear. Solution containing drug and polymer were added drop wise to aqueous phase under continues stirring. The formed nanoparticles suspension were homogenized at 18000 rpm for 15min then followed by magnetic stirring for 3hr. The suspension was centrifuged at 9,000 rpm. for 45 min. The samples were added to glass vials & freeze-dried with mannitol 2% (w/v) as cryprotectant in a lyophilizer. 2.2.2. Total Drug Content (TDC) and Entrapment Efficiency (EE) The total amount of drug per unit volume was determined by suitably disrupting 1ml of the dispersion in 10ml suitable solvent volumetrically. Total drug content was determined by using the equation given below: EE was determined by analyzing the clear supernatant obtained by centrifuging the developed SLN dispersions using Remi Ultracentrifuge. The EE was calculated as follows: Where Df = Amount of drug in clear supernatant fluid. 2.2.3. Particle Size Analysis Nanoparticles formulation was characterized for particle size using Malvern 2000. Double distilled water was used as a dispersant medium. 2.2.4. Particle Shape and Surface Morphology Scanning Electron Microscopy (SEM) analysis of the prepared nanoaprticles was carried out to study the morphology like sphericity and aggregation. Sample was examined by SEM (Jeol, JSM-6360). 2.2.5. FT-IR Spectroscopy Drug was characterized by FT-IR spectroscopy. The spectrum was recorded using FT-IR spectrophotometer (Jasco, FT/IR-4100). The scanning range was 4000 to 400cm-1 . The spectrum of RIF is shown in Figure No. 2. The samples were previously dried and mixed thoroughly with Potassium bromide in 1:5 (Sample:KBr) were obtained at a resolution of 2 cm-1 from 4000 to 400 cm-1 . 2.2.6. Differential Scanning Calorimetry (DSC) DSC measurements were performed on differential scanning equipped with an intra-cooler (DSC Mettler STAR SW 9.01). Inert atmosphere was maintained by purging Nitrogen gas at a flow rate of 50ml/min. RIF and RIF- Nanoparticles, approximately 3-5mg of each sample was heated in aluminium pan from 40 0 C to 240 0 C at heating rate of 10 0 C/min under a stream of Nitrogen at flow rate of 20ml/min. 2.2.7. X-Ray Diffraction (XRD) Study X-Ray diffraction patterns of the powdered samples of the drug RIF and carrier were recorded using Philips PW3710 Analytical XRD B.V. X-Ray diffractometer using CU K 2α-rays with a voltage of 40kV and a current of 25mA. Samples were scanned for 2θ from 5 to 500 C. Diffraction pattern for RIF was obtained. 2.2.8. In vitro Drug Release Study Rifampicin loaded nanoparticles formulation equivalent to drug dose (250 mg) was filled in (size“0”) capsule. The quantitative in vitro release test was performed in two different GI environment i.e. 0.1N HCl (stomach), 6.8 pH buffer. At first two hours, in vitro release test was performed in 900 mL (0.1N HCl). This study was then continued for four hours in 900 ml (6.8 pH buffer solution) maintained at 37 ± 0.5°C using USP type I dissolution apparatus. The basket were rotated at 50 rpm. 5 ml aliquots was collected periodically (30, 60, 90, 120, 150, 180, 210, 240, 270, 300, 330, 360, 390, 420, 450, 480) and replaced with fresh dissolution medium. Aliquots, after filtration through whatman filter paper #45 and diluted . Analysis was carried out using UV spectrophotometer. Results were compared with pure rifampicin. The dissolution experiments were carried out in triplicate, and data were expressed as mean ± S.D.
  • 3. International Journal of Healthcare and Medical Sciences 119 2.2.9. Anti-Microbial Study The antimicrobial study of formulated rifampicin nanoparticles was carried out by using agar gel diffusion method. In which weighed 9 gm of Agar-Agar and 5 gm of nutrient broth mixed it into 300 ml of DW. The prepared nutrient medium placed in Autoclave and start sterilization cycle according to IP 2007, in which holding time becomes 30 min to 60 min at 15 psi pressure and temperature reaches up to 1150 C to 1380 C after completion of cycle, nutrient medium was transferred into sterile petri-plates for cooling. Cultured microorganism Bacilus subtilis (B. subtilis), Staphylococcus aureus (S. aureus) etc. were spread on nutrient medium then the prepared suspension of nanoparticles and pure drug were poured into the well and kept it into the freeze for 20 min. then petriplates were incubated for 12 hrs and finally observed the plates for calculating zone of inhibition. 3. Result & Discussion 3.1. Characterization of RIF-Polymeric Nanoparticles Nanoparticles were prepared using poly methyl methacrylate and Poly vinyl alcohol (Surfactant). The Nanoparticles formulation exhibited a small particle size below 213nm and a TDC of >95% (w/v) with Entrapment efficiency 96.04%. Table-1. Experimental runs with results of response Batch X1 polymer (mg) X2 Surfactant (%) Drug (mg) Y1 Entrapment Efficiency (%) Y2 Particle size (nm) F1 750 1.5 100 91.08 ± 0.23 723 ± 0.43 F2 1000 2.5 100 78.95 ± 0.48 831 ± 0.82 F3 750 2 100 89.82 ± 0.82 527 ± 0.29 F4 1000 2 100 76.8 ± 0.56 713 ± 0.81 F5 500 2.5 100 89.43 ± 0.21 384 ± 1.03 F6 500 2 100 90.67 ± 1.04 324± 0.89 F7 500 1.5 100 92.04 ± 0.63 540 ± 0.39 F8 750 2.5 100 96.04 ± 1.03 213 ± 0.72 F9 1000 1.5 100 80.12 ± 0.87 921 ± 0.41 3.2. Particle Shape and Surface Morphology The morphology of nanoparticles is similar as they appear generally well formed and characterized by a spherical shape. Shown in Figure No. 1 (A) below: Figure-1. (A) SEM of Optimized Formulation F-8, (B) Particle size distribution for Optimized Formulation F-8 3.3. Particle Size The mean particle size of the RIF-Nanoparticles formulation was 213nm showed in Figure No. 1 (B). 3.4. Infrared Spectroscopy IR spectra of pure drug RIF and formulation showed no interaction with the drug and prominent peaks of the drug were not affected. Hence drug-excipients compatibility was established suggesting that there is no interaction between RIF and other excipients or no degradation of drug molecule.
  • 4. International Journal of Healthcare and Medical Sciences 120 Figure-2. FTIR Spectrums of (A) Pure drug RIF, (B) Formulation batch F8 3.5. Differential Scanning Calorimetry DSC of RIF observed has been shown in Figure No. 3. Figure-3. Overlay of DSC curve of Drug and Formulation DSC curve presents an endothermic peak with Tonset at 174.200 C, Tp (temperature of peak) at 191.740 C and Tf (temperature of extrapolated end set) at 198.600 C. The sharp endothermic peak Tp at 191.740 C (actual M.P. 1860 C) corresponds to the melting point of RIF which confirms with value mentioned in the literature. 3.6. X-Ray Diffraction Study As XRD was performed to confirm the findings obtained by DSC, the X-ray patterns of Rifampicin and RIF- Nanoparticles are shown in Figure No. 4.
  • 5. International Journal of Healthcare and Medical Sciences 121 Figure- 4. X-ray Diffraction Patterns of (A) Pure Drug RIF,(B) Optimized Formulation F-8 3.7. In vitro Drug Release Study The in vitro drug release of F8 formulations is shown in Figure No. 5. Figure-5. (A) in vitro drug release profile comparison (B) In vitro drug release graph for F-1 to F-9 From Figure No. 5, In vitro drug releases from formulation F-1 to F-9 were carried out. From the above drug release study it is found that formulation F-8 showed better drug release (90.48%) in 8hrs compared to others. 3.8. Anti-Microbial Study Antimicrobial activity of RIF-Nanoparticles was carried out with the individual component by using agar gel diffusion method. In that method Bacilus subtilis (B. subtilis), Staphylococcus aureus (S. aureus) cultured microorganisms were used. From the Figure No. 6, the zone of inhibition of each component was observed, in that zone of inhibition of formulation and the pure drug were clearly observed. The above observation might be concluded that the RIF-Nanoparticles had great antimicrobial potential which may further apply for various medical applications.
  • 6. International Journal of Healthcare and Medical Sciences 122 Figure-6. Antimicrobial activity of RIF-Nanoparticles on microorganism (A) B. subtilis, (B) S. aureus (A) (B) Table-2. Observation Table for Microbial Assay Microorganism Diameter Plain Drug Formulation Staphylococcus aureus 3.2 ± 0.05cm 3.5 ±0.23 cm 3.3 ± 0.15cm 3.6 ±0.057 cm 3.2 ± 0.057cm 3.6 ± 0.20 cm Bacilus subtilis 2.5 ± 0.15cm 2.9 ± 0.15cm 2.1 ±0.15cm 2.7 ± 0.208cm 2.2 ± 0.15cm 2.3 ± 0.15cm 4. Conclusion In the present study, polymeric nanoparticles of Rifampicin were developed to a satisfactory level in terms of particle size, drug entrapment, drug release and antimicrobial activity. The particles were found to be spherical and smooth. The drug release data shows satisfactory results when compared with drug and marketed formulation. The antimicrobial study shows good zone of inhibition when compared with plain drug. So these drug delivery systems have potential to treat tuberculosis. References [1] Vyas, S. P., Kannan, M. E., Jain, S., Mishra, V., and Singh, P., 2004. "Design of liposomal aerosols for improved delivery of rifampicin to alveolar macrophages." Int. J. Pharm, vol. 269, pp. 37–49. [2] Shokri, N., Akbari, J. H., Fouladdel, S. H., Khalaj, A., Khoshayand, M. R., and Dinarvand, R., 2011. "Preparation and evaluation of poly (caprolactone fumurate) nanoparticles containing Doxorubicin HCL." DARU, vol. 19, pp: 12-22 [3] Abhilash, M., 2010. "Potential applications of Nanoparticles." Int J Pharm Bio Sci., vol. 1, pp: 1-12 [4] Kayser, O. A. L. and Hernández-Trejo, N., 2005. "The Impact of nanobiotechnology on the development of new drug delivery systems." Current Pharmaceutical Biotechnology, vol. 6, p. 35.