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Facile preparation of acrylamide grafted locust bean gum-poly(vinyl alcohol) interpenetrating polymer network microspheres for controlled oral drug delivery
Accepted Manuscript Facile preparation of acrylamide grafted locust bean gum-poly(vinyl alcohol) interpenetrating polymer network microspheres for controlled oral drug delivery Santanu Kaity, Animesh Ghosh PII:
S1773-2247(16)30045-4
DOI:
10.1016/j.jddst.2016.02.005
Reference:
JDDST 169
To appear in:
Journal of Drug Delivery Science and Technology
Received Date: 18 December 2015 Revised Date:
2 February 2016
Accepted Date: 19 February 2016
Please cite this article as: S. Kaity, A. Ghosh, Facile preparation of acrylamide grafted locust bean gumpoly(vinyl alcohol) interpenetrating polymer network microspheres for controlled oral drug delivery, Journal of Drug Delivery Science and Technology (2016), doi: 10.1016/j.jddst.2016.02.005. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT
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Am-g-LBG
Am-g-LBG-PVA blend
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PVA
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Emulsion crosslinking
IPN microspheres
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For graphical abstract only
Controlled release of BH
ACCEPTED MANUSCRIPT ORIGINAL RESEARCH ARTICLE
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Facile preparation of acrylamide grafted locust bean gum-poly(vinyl alcohol)
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interpenetrating polymer network microspheres for controlled oral drug delivery
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Santanu Kaity and Animesh Ghosh*
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Department of Pharmaceutical Science and Technology, Birla Institute of Technology,
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Mesra, Ranchi- 835215, Jharkhand, India.
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* Corresponding author:
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Department of Pharmaceutical Sciences and Technology
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Birla Institute of Technology, Mesra
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Ranchi – 835215, Jhakhand, India.
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Tel.:+91-9470339587, Fax-+91-6512275290
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Email address: [email protected] (Animesh Ghosh)
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ACCEPTED MANUSCRIPT Abstract:
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Hybridization of natural and synthetic polymers is used to improve the physicochemical
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stability, swelling and drug release pattern of the respective materials in biological condition.
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In present study, a biodegradable, biocompatible and stable interpenetrating polymer network
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(IPN) of acrylamide grafted locust bean gum (Am-g-LBG) and poly(vinyl alcohol) (PVA)
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was developed by emulsion crosslinking method for spatial and temporal drug delivery. The
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IPN microspheres were prepared with the help of glutaraldehyde as a crosslinker for
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controlled oral delivery of buflomedil hydrochloride. The formulation parameters were
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optimized in terms of different gum:PVA ratio, crosslinker amount and drug loading. The
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microspheres were evaluated for their drug entrapment efficiency, particle size, swelling,
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SEM, FTIR, NMR, DSC, XRD and in vitro drug release profile. The particles showed well
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controlled release characteristics and continued to drug release following diffusion controlled
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release pattern. The drug release was for prolong time without collapsing the particle matrix.
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Thus, IPN microspheres based delivery system can be a better approach for controlled
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delivery of highly water soluble drugs like buflomedil hydrochloride.
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Key words: Controlled release; Acrylamide grafted locust bean gum; Poly(vinyl alcohol);
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Buflomedil hydrochloride; Interpenetrating polymer network.
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ACCEPTED MANUSCRIPT 1. Introduction:
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The prime aim of controlled release drug delivery is “spatial placement” and “temporal
43
delivery”. Spatial placement refers to drug targeting to specific organs, tissue cells or even
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sub-cellular compartments; whereas, temporal delivery refers to control the rate of drug
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delivery to the target site.
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system can be a major advance towards delivering the drug molecules to their intended
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destination. Multi-particulate delivery systems have gained special interest because of their
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capability to meet the needs of spatial and temporal delivery of drug molecules with
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minimum fluctuation of plasma drug concentration. [2]
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An interpenetrating polymer network (IPN) is a composite of two polymers, which obtained
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when at least one polymer network is synthesized or cross-linked independently in the
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immediate presence of the other.
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improve mechanical properties and thermal stability.
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polymer based network systems has extensively studied for drug delivery purpose as they are
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biodegradable, biocompatible and can be tailored as intended.
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polymer combination of natural and synthetic origin has been found to be useful to control
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the release of short half-lived drugs under physiological conditions. [7]
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Recently, a large number of IPN microspheres have been developed using different polymer
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combinations for drug delivery purpose. Among them, Poly(vinyl alcohol) (PVA) based IPN
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systems are extensively studied
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biocompatibility and desirable physical properties such as sufficient mechanical strength and
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high degree of swelling in aqueous solution. [12] A combination of PVA with natural polymer
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may provide the system with better stability and improved mechanical strength to meet the
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major objectives of controlled release drug delivery.
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A strategically developed controlled release drug delivery
Chemical crosslinking between these polymers leads to [4]
In majority of the cases, the natural
[5, 6]
A judicially selected
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[8-11]
due to its inherent non-toxicity, non-carcinogenicity,
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Various natural polymers have been explored for controlled-release microspheres
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development. Among them, guar gum, [10, 11] xanthan gum, [3] gellan gum, [9] locust bean gum,
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[13]
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acrylamide grafted locust bean gum and PVA was selected as matrix for IPN based
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microspheres development. To make a multi-particulate delivery system which will be able to
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deliver the API for prolong time, the delivery device should have sufficient integrity during
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its GI residence. This hybridization was selected to make the matrix crosslinkable and to
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provide sufficient integrity to the particulate delivery device during its GI residence.
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Locust bean gum (LBG) is a high molecular weight branch polysaccharide and is extracted
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from the seeds of carob tree Ceratonia siliqua. It is a non-starch polysaccharides consisting
75
of galactose and mannose in the ratio of 1:4 and hence they are known as galactomannan. [15]
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LBG is consists of (1,4)-linked β-D mannopyranose backbone with branch points from their
77
6-positions linked to α-D-galactose. The molecular weight of LBG ranges between 300,000
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and 1,200,000 Da. It is not easily soluble in water due to relatively hydrophobic nature of
79
mannan unit and requires heating to affect solvation. [16]
80
Recently, we have explored the efficiency of native LBG and carboxymethylated LBG
81
(CMLBG) with PVA as IPN controlled release drug delivery device.
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observed poor entrapment efficiency of the particles. Moreover, in case of native LBG we
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observed miscibility problem with aqueous PVA solution. Grafting of polyacrylamide onto
84
LBG can increase the aqueous solubility of resultant polymer.
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grafted LBG and PVA may be able to overcome the problems observed in case of LBG-PVA
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and CMLBG-PVA IPNs. So, in present study, IPN microspheres of acrylamide grafted locust
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bean gum (Am-g-LBG) and PVA was prepared for controlled oral delivery of a highly water-
88
soluble drug, buflomedil hydrochloride (BH). BH is readily absorbed in the gastrointestinal
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tract and has a plasma half-life of approximately 2 to 3 h. The usual oral dose of BH is 300 to
[14]
has been reported till date. In present study, a novel combination of
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chitosan
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[13, 17]
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IPN with acrylamide
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600 mg/day. Long-term use of BH in high doses can produce drug accumulation and drug
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related toxicity.
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BH, can reduce the dose and dose related side effects.
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The IPN particles of Am-g-LBG and PVA were developed by emulsion crosslinking method
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and the microspheres were evaluated for their drug entrapment efficiency, particle size,
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swelling, scanning electron microscopy (SEM), Fourier transform infrared spectroscopy
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(FTIR), nuclear magnetic resonance (NMR) spectroscopy, differential scanning colorimetry
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(DSC) and X-ray diffraction (XRD) profile. An in vitro drug release study [in both acidic
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media (pH 1.2) and phosphate buffer (pH 6.8)] and kinetic modelling was performed to
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understand the drug release mechanism.
Therefore, a controlled-release approach, such as IPN microspheres of
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2. Materials:
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Buflomedil hydrochloride was obtained as gift sample from Fresenius Kabi Oncology
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Limited (Kalyani, West Bengal, India). Locust bean gum and poly(vinyl alcohol) (PVA;
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average molecular weight 125000 Da) were purchased from HiMedia Laboratories Pvt. Ltd.
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(Mumbai, India). Light liquid paraffin (LLP; viscosity 25−80 mPa at 20°C), hydrochloric
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acid (HCl; 30%, ultra-pure) and acetone (Density = 0.789 to 0.791 g/mL) were obtained from
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Rankem India Pvt. Ltd. (Mumbai, India). Span 80 was procured from Pioneer In-Organics
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(Delhi, India). Glycine and glutaraldehyde (GA; 25%, v/v) were supplied by Merck India
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Ltd. (Mumbai, India). All the reagents were used without further purification. Water used
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was of Milli-Q grade.
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3. Methods:
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3.1. Synthesis of acrylamide grafted locust bean gum (Am-g-LBG)
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acrylamide grafted LBG. [18] In brief, 10 g of acrylamide (Am) was dissolved in 30 mL water
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and mixed with 120 mL aqueous dispersion of LBG (0.0083g/mL). 300 mg ceric ammonium
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nitrate (CAN) was dissolved in 30 mL of water and mixed with the Am-LBG mixture. The
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dispersion was irradiated by microwave (Laboratory scientific microwave system, Catalyst
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systems, India) at 480 W for 2.5 min. using alternate one minute heating and cooling cycle.
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The grafted gum was precipitated using acetone and washed with absolute and 30% aqueous
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ethanol. The grafted gum thus prepared was vacuum dried at 40⁰C to a constant weight and
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converted to fines for further use.
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3.2. Preparation of Am-g-LBG-PVA IPN microspheres
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Buflomedil hydrochloride (BH) entrapped IPN microspheres of PVA and Am-g-LBG were
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developed by water-in-oil (w/o) emulsion-crosslinking method (Figure 1). [14] Briefly, 20 mL
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of 2% (w/v) aqueous polymeric solution (total polymer amount was kept constant) was
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prepared by dispersing varying amounts of Am-g-LBG in aqueous PVA solution. The
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required amount of BH was added in the polymeric dispersion. The drug- polymer blend was
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slowly emulsified with light liquid paraffin (100 g) containing 1% (w/w) Tween-80 under
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constant mechanical stirring (IKA Labortechnik, Staufen, Germany) at 500 rpm. A milk
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white emulsion (w/o) was obtained. To this emulsion, GA (2.5 and 5 mL) containing 0.5 mL
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of 1 N HCl was added slowly and stirring was continued for 3 h. The crosslinked
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microspheres were then filtered and washed with acetone, 0.1 M glycine solution and water to
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remove excess amount of liquid paraffin, unreacted GA and surfactant, respectively.
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Complete removal of unreacted GA was confirmed by treating the filtrate with Fehling’s
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reagent. A negative result assured the absence of unreacted GA. Hardened microspheres were
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vacuum-dried at 40°C for 24 h and stored in desiccator until further use. The absence of
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crushed dried particles and treating it in similar way as said earlier.
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For the preparation of blank microspheres similar method was adopted except the addition of
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drug into the system. Detailed formulation variables are given in Table 1.
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Insert Table 1 here.
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Insert Figure 1 here.
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3.3. Full factorial design
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In the present study, two-level [high level (+1) and low level (−1)], three-factor, full factorial
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design (8 batches) was used for the optimization of gum:PVA ratio, crosslinker and drug
146
loads (independent variables). The responses (dependent variables) selected for optimization
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were drug entrapment efficiency, particle size, swelling and cumulative percentage drug
148
release in dissolution study. The results (Tables 1) of response generated using the
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experimental designs were analysed by factorial models using Design Expert software
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(Version 7.0.0, Stat-Ease, Inc., Minneapolis). The 3D response plots are presented in Figure
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2.
152
Insert Figure 2 here.
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3.4. Fourier transform infrared spectroscopy (FTIR)
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The FTIR spectrums of Am-g-LBG, PVA, BH, drug-polymer physical mixture, blank
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microspheres, and drug loaded microspheres were carried out by FTIR-8400S (Shimadzu,
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Japan) to confirm the formation of Am-g-LBG and compatibility of different ingredients of
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the IPN formulations. A small amount of each material was mixed with potassium bromide
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(KBr) (1 %w/w sample content), taken into sample holder and scanned in the range of 600 to
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4000 cm-1.
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Solid state 13C NMR of Am-g-LBG, PVA and glutaraldehyde crosslinked blank formulation
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was studied to confirm the formation of Am-g-LBG and glutaraldehyde crosslinked IPN
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network. For solid state 13C NMR, approximately 300 mg of samples were inserted into the
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ceramic rotor on a Bruker AMX 400 spectrometer. The spectrum was recorded at 75.5 MHz.
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3.6. Differential scanning calorimetry (DSC)
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DSC thermograms of Am-g-LBG, PVA, BH, blank formulation and drug loaded formulations
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were obtained by using DSC-60 (Shimadzu, Japan). Each sample (3–7 mg) was accurately
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weighed into a 40 µL aluminium pan in a hermetically sealed condition. The measurements
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were conducted in nitrogen atmosphere between 30°C and 350°C at the heating rate of
170
10°C/min. The Am-g-LBG and the drug loaded formulations were heated in-situ up to 110⁰C
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to make them moisture free. Then the samples were cooled to room temperature and reheated
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up to 350⁰C.
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3.7. Qualitative X-Ray diffractometry (XRD)
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Grinded samples of blank IPN microspheres, drug loaded IPN microspheres, BH were
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scanned from angular range of 10° to 60° 2θ, using an X-ray diffractometer (Bruker AXS D8
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Advance, Germany, Configuration: Vertical, Theta/2 Theta geometry: X-ray Cu, wavelength
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1.5406 A°, Detector: Si (Li) PSD. The diffractometer was run at a scanning speed of 2°/min
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and a chart speed of 2°/2 cm per 2θ.
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3.8. Scanning electron microscopy (SEM)
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The surface morphology and topography of Am-g-LBG-PVA IPN microspheres were
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evaluated by scanning electron microscope (JSM-6390LV, Jeol, Japan). Before examination,
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vacuum coated with gold palladium film (thickness 2 nm) by sputter coater (Edward S-150,
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U.K.) to make them electrically conductive. Representative sections were photographed for
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evaluation.
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3.9. Drug encapsulation efficiency (DEE)
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IPN particles were crushed in mortar and pestle and a specified amount (10 mg) was taken
188
into 50 mL of phosphate buffer solution (pH 6.8), heated at 50°C for effective drug
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extraction. After 24 h, the suspension was subjected for filtration and centrifugation for the
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removal of polymeric debris. The supernatant was analysed with a spectrophotometer (UV-
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1800, Shimadzu, Japan) at λmax of 282 nm. All samples were analysed in triplicate. The drug
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entrapment efficiency (%) was calculated by using the following equation: [20]
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Encapsulation efficiency (%) = (Actual drug content / Theoretical drug content) × 100
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(1)
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3.10. Swelling study
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Equilibrium swelling study of IPN microspheres was done in different media. An accurately
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weighed amount of microspheres (W1) was immersed in 50 mL buffer (pH 1.2 and pH 6.8)
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and allowed to swell for 24 h at 37°C.The swollen microspheres was collected and the
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adhered liquid droplets on the surface of the particles was removed carefully with tissue
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paper and reweighed (W2) to an accuracy of ±0.01 mg on an electronic microbalance
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(Mettler, model AT120, Greifensee, Switzerland). The swelling index was calculated by the
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formula given below: [11]
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Swelling index = [(W2-W1) / W1]× 100
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Where, W2 and W1 are the swollen and dry weights of the gum/microspheres, respectively.
Eq.
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Eq. (2)
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Particle size of IPN microspheres were determined by using a Mastersizer 2000 Ver.5.40
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(Malvern Instruments Ltd., UK) which allows sample measurement in the range of 20–2000
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µm. The micro particles were dispersed in water and the size was measured using the laser
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light scattering technique. Polydispersity index (PDI) was determined according to the
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equation:
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Polydispersity index = [d(0.9) – d(0.1)]/d(0.5)
Eq. (3)
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where, d(0.9), d(0.5) and d(0.1) are the particle diameters determined respectively at the 90th,
213
50th and 10th percentile of undersized particles. [21]
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3.12. In vitro drug release and release kinetic study
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In vitro drug release from the IPN microspheres were investigated in pH 1.2 for the initial 2
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h, followed by phosphate buffer of pH 6.8. All the experiment was performed in triplicate in
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a dissolution tester (Electro Lab, TDT-08L, India) equipped with eight baskets (glass jars) at
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the stirring speed of 50 rpm. An accurately weighed quantity of each sample (equivalent to
219
100 mg BH) was placed in 900 mL of dissolution medium maintained at 37.5⁰C. At regular
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intervals of time, sample aliquots were withdrawn and analysed using UV spectrophotometer
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(UV-1800, Shimadzu, Japan) at the fixed λmax of 282 nm.
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The release data were fitted in various empirical equations like Zero order (Qt = Kt), First
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order (ln Qt= ln Q0-Kt ), Higuchi kinetic (Qt= Ktn), Hixson-Crowell (Q01/3- Qt1/3 = Kt) and the
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power-law equation: Mt/M∞ = ktn, where Mt/M∞ is the fraction of drug release at time t, k is
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the release rate constant, and n is the diffusion exponent that denotes the drug-release
226
mechanism. [22] A least squares regression method was used to determine the values of n and
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k. Values of n = 0.43 or less indicate Fickian transport, whereas values of n of 0.43–0.85
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signifies the super case II transport mechanism.Q0 and Qt are amount of drug released at zero
230
and t time. K represents release rate constant.
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4. Results and discussion:
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The microwave assisted grafting method was used in present study to induce rapid energy to
233
the reaction system and to reduce the reaction time. The ceric ion from CAN generates free
234
radical sites on LBG backbone (Figure 3). LBG free radicals used to couple with acrylamide
235
by covalent linkage. The reaction is terminated by coupling of two free radicals.
236
details of synthetic parameters of IPN microspheres are given in Table 1. Acrylamide is an
237
excellent monomer which is freely soluble in water and can be mixed with hydrophilic gum
238
solution to make a homogenous blend. Thus it can easily attach with the adjacent gum
239
backbone by free radical polymerization thus reduce the chance of high amount of
240
homopolymer formation. Moreover acrylamide in low dose is non-toxic, easily excreted from
241
body and plasma half life is very less (2-2.5 h). The method of IPN particle preparation and
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proposed reaction mechanism of IPN formation is shown in Figure 1 and Figure 3,
243
respectively. The general mechanism of matrix crosslinking with GA, a bi-functional
244
crosslinker, was through developing an acetal ring between the hydroxyl groups of Am-g-
245
LBG and PVA with the aldehyde groups of GA. This aided the formation of the IPN
246
microspheres in the emulsion phase. [14]
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Insert Figure 3 here.
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4.1. Fourier transform infrared spectroscopy (FTIR)
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The FTIR spectral study of Am-g-LBG, buflomedil hydrochloride, PVA, physical mixture,
250
blank microspheres and optimized drug loaded microspheres (Figure 4) was performed to
[18]
The
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of Am-g-LBG and GA crosslinked IPN matrix structure.
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As presented in Figure 4, the Am-g-LBG showed the bands at 1683 and 1651 cm-1 were
254
attributed to amide-I (C–O stretching) and amide-II (N–H bending) conferred by Am. [23] The
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peak at 2800–3566 cm−1 in Am-g-LBG was due to overlap of N–H stretching band of amide
256
group and O–H stretching band. A band at about 1454 cm−1 was due to the C–N stretching.
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Peak at 1010 cm−1 was attributed to CH-O-CH2 group which occurs during grafting reaction
258
between OH group of C2 and π bond of acrylamide.
259
evidenced that LBG was successfully modified to Am-g-LBG.
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For buflomedil hydrochloride major peaks were observed at about 2968 cm−1 for methoxy
261
CH stretching (CH3-O-). A small peak at about 1339 cm−1 was observed for aromatic C-N
262
stretching. Absorption band at 1701 cm-1 was of ketonic carbonyl group (Figure 4).
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In case of PVA major peaks related to hydroxyl and acetate groups were present in FTIR
264
spectra. The large band observed between 3600 and 3200 cm−1 are linked to the O–H
265
stretching of the intermolecular and intramolecular hydrogen bonds. The vibrational band
266
observed between 2854 and 2944 cm−1 referred to the C–H stretching from alkyl groups and
267
the peaks between 1740–1716 cm−1 were due to the stretching C=O and C–O from acetate
268
group residues from PVA (Figure 4). A sharp peak obtained near 1456 cm-1 indicated the
269
bending vibration of CH2 groups. The intensity of the 1740– 1716 cm−1 strongly suggested
270
that it was less hydrolysed. [24]
271
The physical mixture showed the peaks of all components (BH, PVA and Am-g-LBG) in its
272
spectra without significant changes, indicating compatibility of the ingredients. The peak
273
intensities were observed to be reduced for all components due to the dilution effect.
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FTIR analysis of Am-g- LBG
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In the placebo Am-g-LBG-PVA IPN formulation, a considerable intensity reduction of the
275
O–H peaks from the PVA was noted, giving a possible indication of acetal bridge formation.
276
[25]
277
to ether linkage (C-O-C stretching) formed between the –OH group of PVA and Am-g-LBG
278
by the help of glutaraldehyde. [10] Peaks near about 1735 and 1650 cm −1 may be due to C=O
279
group of PVA acetate and amide-II (N–H bending) conferred by Am-g-LBG, respectively
280
(Figure 4). Thus, it can be said that Am-g-LBG and PVA was successfully crosslinked by GA
281
to form the network structure.
282
The drug loaded microspheres showed the additional peaks of BH in FTIR spectra than that
283
of placebo microspheres. Peaks at about 2925 cm−1 (methoxy CH stretching), 1338 cm−1
284
(aromatic C-N stretching) and 1702 cm-1 (ketonic carbonyl group) were due to BH (Figure 4).
285
No additional peaks were observed in the drug incorporated formulation than that of BH and
286
formulation components indicating that the ingredients itself and the process was compatible
287
for the preparation of BH loaded Am-g-LBG-PVA IPN microspheres.
288
Insert Figure 4 here.
289
4.2. Solid state 13C NMR spectroscopy
290
As per the earlier reports, the major peaks in the 13C NMR spectrum of LBG observed at δ =
291
62.0 ppm for the C-6 carbon of mannan unit, δ = 70-80 ppm for the signals of C-2, C-3 and
292
C-5 carbon atom, δ = 81.0 ppm for the C-4 mannan carbon atom and a sharp peak at δ =
293
102.7 ppm for C-1 mannan carbon atom. [13]
294
In the
295
CH2-CH-)n groups, formed due to Am polymerization, peak at δ=180.8 ppm for carbon atoms
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A small absorption peak at about 1250 cm −1 was observed in the spectrum which was due
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C NMR spectrum of Am-g-LBG (Figure 5), the peak at δ=42.5 ppm was for (-CH-
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297
Am-g-LBG.
298
The NMR spectrum of PVA consists of one broad peak at 45.8 ppm due to the methylene
299
carbon and a group of three peaks at δ = 62.8, 72.9, and 82.6 ppm from the oxymethine
300
carbon (Figure 5).
301
The
302
42.2 ppm due to the (-CH-CH2-CH-)n groups of acrylamide polymerization. The absorption
303
peak at δ = 61.3 ppm and 72.8 ppm are for PVA methine carbon. Peak at δ = 101.9 ppm is
304
due to the acetal carbon atom
305
group due to cross linking by glutaraldehyde proves the formation of IPN (Figure 5). The
306
broadened peak at δ = 177.4 ppm is for carbon atoms of –CONH2 group. Hence, the solid
307
state NMR spectra of the IPN particles showed a strong evidence of formation of
308
glutaraldehyde crosslinked IPN matrix of Am-g-LBG and PVA.
309
Insert Figure 5 here.
310
4.3. Differential scanning calorimetry (DSC)
311
From the DSC study it was observed that the Am-g-LBG showed its transition mid point
312
temperature (Tm) at about 238⁰C (Figure 6). It was almost similar as reported earlier. [18] PVA
313
showed its characteristic melting peak at about 192⁰C and a degradation peak was observed
314
at about 322⁰C (Figure 6). In case of pure BH, a sharp melting peak was observed at about
315
197⁰C which was matching with previous reports. [13] In case of placebo microspheres, peaks
316
due to individual components were hard to detect. However, a broad endothermic peak was
317
observed at about 288⁰C. This may be an indication of formation of a polymer composite
318
which degrades at a temperature other than the degradation points of individual basic
[17]
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which formed between the Am-g-LBG and PVA hydroxyl
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ACCEPTED MANUSCRIPT components. In drug loaded formulation, the endothermic peak at about 196⁰C was due to the
320
melting of entrapped BH (Figure 6). A broad endothermic peak was observed at about 278⁰C
321
which may be due to the degradation of the Am-g-LBG-PVA composite network structure.
322
Thus, from DSC study it can be said that a complex network structure was formed between
323
Am-g-LBG and PVA crosslinked by GA. Moreover, BH was successfully encapsulated in the
324
IPN polymer matrix.
325
Insert Figure 6 here.
326
4.4. Qualitative X-Ray diffractometry (XRD)
327
From the diffractogram of BH (Figure 7), it can be said that, it is highly crystalline in nature.
328
BH showed its characteristic peaks at 2θ of 6-50⁰. Sharp intense peak at about 2θ of 6⁰, 15⁰
329
and 21⁰ proves its crystalline nature. Drug loaded microspheres showed a broad peak at about
330
2θ of 20⁰. However, other peaks have disappeared in BH loaded microspheres assuring that
331
drug is molecularly dispersed in the polymer matrix. The peak intensity at 2θ of 20⁰ is higher
332
in drug loaded formulation than that of placebo confirms the presence of BH in IPN matrix.
333
Insert Figure 7 here.
334
4.5. Scanning electron microscopy (SEM)
335
The SEM image reveals surface morphology of the IPN particles and represented in Figure 8.
336
The particles which were prepared by PVA only (A9, Figure 8a) were having smooth surface
337
and well defined spherical structure. The particles prepared by Am-g-LBG and PVA in
338
combination with less amount of GA (Figure 8b) showed some pores on the surface.
339
However, the particles prepared with high amount of GA were appeared to be solid and there
340
was no pore on the surface (Figure 8c). This happened because of the higher crosslinking of
341
the polymer matrix. The surface appeared to be tough and showed evidence of network
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15
ACCEPTED MANUSCRIPT structure (Figure 8d). The cross sectional view of microspheres (Figure 8e and 8f) also
343
showed a strong evidence of the formation of well-defined polymer network structure.
344
Insert Figure 8 here.
345
4.6. Drug encapsulation efficiency (DEE)
346
The drug entrapment efficiency of Am-g-LBG-PVA IPN microspheres (Table 1) was
347
observed in the range of 51.32±1.94 (A2) to 73.51±2.78% (A1).This improvement in DEE
348
was due to the optimum miscibility of two phases and the highly branched structure of the
349
grafted gum which prevented the leaching of drug during the crosslinking stage. [18] The drug
350
entrapment capacity was observed to be dependent on the gum:PVA composition, crosslinker
351
and drug loads. A higher amount of Am-g-LBG (formulation code A2 - A5) led to reduced
352
DEE due to increased hydrophilicity of the system and inability of crosslinker to crosslink the
353
total system (Table 1). Similar findings were reported by Sullad et al. (2010).
354
increased amount of GA helped in higher drug entrapment due to the formation of rigid
355
polymer matrix (A1 and A6). Interestingly an increased drug loading showed least effect on
356
the DEE of the IPN microspheres (A1 and A8). This may be due to the saturation of the
357
matrix by the optimum drug concentration.
358
The three dimensional plot of the effects of different formulation variables on %DEE is
359
shown in Figure 2a. The mathematical relationship of DEE with the independent variables
360
was generated by MLRA and expressed as:
361
[11]
An
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DEE (%) = 63.58+6.29A+3.48B+1.35C
Eq. (4)
362
Where, A is gum:PVA ratio, B is glutaraldehyde amount and C is % drug loading. Here we
363
observed that all the independent variables were having positive impact on %DEE as was
364
observed experimentally. ANOVA analysis indicated that the model was significant (P < 16
ACCEPTED MANUSCRIPT 0.05) with R2 value 0.99. The adjusted (0.98) and predicted (0.96) R2 were reasonably in
366
good agreement.
367
4.7. Swelling study
368
The swelling of Am-g-LBG-PVA IPN microspheres (Table 1) was observed to be moderately
369
pH dependent. The extent of crosslinking played a major role in swelling of the microspheres.
370
Highly crosslinked particles (prepared with high amount of GA) showed less swelling (A1,
371
A3, A4 and A8) due to the absence of free hydrodynamic volume in their matrix. The
372
presence of higher amount of grafted gum in microspheres matrix resulted in higher swelling
373
(A2 in pH 1.2 and 6.8, respectively) (Table 1). This happened because of the hydrophilic
374
nature of the grafted gum. This postulation was further confirmed by the swelling
375
characteristics of microspheres having only PVA (A9) which showed least swelling in both
376
the media since it was devoid of grafted gum. The swelling of particles in acidic media (pH
377
1.2) was less in all cases than that of phosphate buffer (pH 6.8). Under pH 6.8, the presence
378
of ionisable groups in the component polymers which deprotonated and exhibited higher
379
swelling ratio due to the collective electrostatic repulsion forces between the ionized groups.
380
[26]
381
A slight increase in swelling was observed in case of formulation having higher drug loading
382
(A3 and A4). This was due to the increased hydrophilicity of the matrix in presence of highly
383
hydrophilic BH.
384
The effects of formulation variables on swelling as observed from MLRA are shown in
385
Figure 2c, 2d and expressed as:
386
Swelling% (pH 1.2) = 255.36 - 13.34A - 14.33B
387
Swelling % (pH 6.8) = 332.93 - 11.27A - 9.91B
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17
Eq. (5) Eq. (6)
ACCEPTED MANUSCRIPT Where, A is gum: PVA ratio and B is GA amount. ANOVA analysis indicated that the
389
factorial model was significant (P < 0.05) having R2 value of 0.91 and 0.92 for pH 1.2 and
390
pH 6.8, respectively. The adjusted (0.88 for both pH 1.2 and 6.8) and the predicted (0.78 and
391
0.79 for pH 1.2 and pH 6.8, respectively) R2 values were in reasonably good agreement. Here
392
both the gum: polymer ratio and GA showed negative effect and drug loading (%) showed
393
negligible influence on swelling as observed experimentally.
394
4.8. Particle size analysis
395
The arithmetic mean diameter of IPN particles varied from 371.06 µm to 766.06 µm (Figure
396
9, Table 1). In a fixed IPN blend composition, higher crosslinker amount resulted in
397
reduction of particle size (For A1 particle size is 449.46 µm, for A6 size is 519.36 µm). This
398
was due to the fact that as the amount of crosslinker was increased, the density of the polymer
399
matrix increased to a higher extent and reduced the internal void space.
400
The particle size was observed to be increased with the amount of Am-g-LBG (For A1
401
particle size was 449.46 µm, for A3 size was 608.76 µm) (Table 1). This can be explained on
402
the basis of hydrodynamic viscosity concept, i.e., with increased Am-g-LBG amount, the
403
interfacial viscosity of the polymer droplets in the emulsion was increased and resulted in the
404
formation of larger particles.
405
An increased drug loading (For A1 and A8 particle size was 429.70 µm and 449.46 µm
406
respectively) also resulted in the formation of bigger particles (Figure 9). The reason behind
407
this was, drug molecules might have hindered the inward shrinkage of the polymer matrix by
408
occupying the free volume spaces within the matrix. The polydispersity index of the Am-g-
409
LBG particles was less and it was in the range of 0.82 and 1.32 (Table 1). This result
410
indicates that the particles formed are of narrow size distribution range.
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18
ACCEPTED MANUSCRIPT 411
The effects of independent variables on the particle size are shown in Figure 2b. The
412
mathematical relationship is expressed as:
413
Particle size = 557.60 – 88.94A – 47.64B
414
Where, A is gum:PVA ratio and B is GA amount. ANOVA analysis indicated that the model
415
was significant (P < 0.05) with R2 value 0.87. The adjusted (0.83) and predicted (0.69) R2
416
were almost in good agreement. Here also we observed the negative effect of gum: PVA
417
ratio and GA on the size of IPN particles. It was in good agreement with experimental
418
observation.
419
Insert Figure 9 here.
420
4.9. In vitro drug release and release kinetic study
421
The cumulative percentage drug release vs. time plot of different batches of Am-g-LBG-PVA
422
IPN microspheres are presented in Figure 10. It was observed that the drug release from the
423
IPN microspheres were dependent upon major factors like crosslinker amount, polymeric
424
blend ratio and to less extent on the amount of drug loading.
425
Effect of crosslinker: In fixed formulating parameters, when the amount of crosslinker was
426
increased from 2.5 mL to 5 mL, the amount of drug release was decreased. In formulation A1
427
and A6 polymer composition (1:2) and drug loading (50%) was same but amount of
428
crosslinker was different. A1 showed less drug release (64%) than A6 (68%) (Figure 10).
429
This may be due to the higher crosslinking of the matrix which prevent solvent imbibition
430
and network erosion leading to high release retardant property.
431
Effect of gum:PVA blend ratio: When the blend ratio of IPN particles were changed from 1:2
432
to 1:1 in fixed crosslinker and drug loading percentage, the drug release increased from 64%
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Eq. (7)
19
ACCEPTED MANUSCRIPT (A1) to 79% (A3) and 68% (A6) to 87% (A2). This was due to the hydrophilic nature of the
434
grafted gum which interacted with media to swell and erode in a faster rate and helped in
435
faster drug release. Particles composed of only PVA (A9) showed 74% drug release in 12 h
436
(Figure 10).
437
Effect of drug loading: Formulations, having different drug loading in a fixed gum: PVA
438
ratio and crosslinker amount, showed different extent of drug release. For example, A2 (25%
439
drug loading, 87% drug release) showed retarded drug release property than A5 (50% drug
440
loading, 93% drug release) (Figure 10) though other parameters for both the formulations
441
were same. It may be due to the reason that, concentration gradient, the driving force, will be
442
high in high drug load formulations and promoted faster drug release. Moreover, low drug
443
load matrix would have a greater gum and polymer fraction to act as the barrier to drug
444
release.
445
The effect of formulation variables on CPR is shown in figure 2e and the mathematical
446
relation is expressed as:
447
CPR = 75.90 - 9.08A – 4.18B
448
Where, A is gum:PVA ratio and B is amount of GA. ANOVA analysis indicated that the
449
model was significant (P < 0.05) with R2 value 0.95. The adjusted (0.93) and predicted (0.88)
450
R2 were in good agreement. The effect of gum: polymer ratio and GA was similar to that of
451
experimental evidence.
452
After generating the model polynomial equations to relate the dependent and independent
453
variables, the best optimized amount of independent variables was finalized in terms of
454
maximum gum: PVA ratio, minimum amount of crosslinker and maximum drug loading to
455
achieve the dependent variables in terms of maximize DEE%, particle size in range,
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20
ACCEPTED MANUSCRIPT maximize swelling and minimum CPR. The software generated solution was in good
457
agreement with batch A6.The optimized Am-g-LBG-PVA IPN particles showed 68.08% drug
458
release at 12 h.
459
Release kinetic: The invitro release data were fitted in different empirical equations and
460
presented in Table 2. It was observed that the best fit was with Higuchi release kinetic,
461
suggesting that the release of drug molecules from IPN matrix was diffusion controlled. The
462
drug release data were also fitted with the Power law equation and the values of n varied
463
from 0.845 to 1.078. For A4 drug release was non Fickian and for the rest the release pattern
464
followed super case II transport mechanism.
465
Insert Figure 10 here.
466
Insert Table 2 here.
467
5. Conclusion:
468
In present study Am-g-LBG-PVA IPN microspheres were successfully prepared by emulsion
469
crosslinking method by using glutaraldehyde as a crosslinker. Among various formulations
470
the A6 batch was the optimized formulation. The particles were spherical with narrow size
471
distribution. The particle showed promising controlled release property with moderate pH
472
sensitivity. This type of polymeric composites may be fruitful as a promising biomaterial to
473
solve the major loop holes of controlled release of highly water soluble drugs with short half
474
life.
475
Conflict of interest:
476
The authors report no conflicts of interest. The authors alone are responsible for the content
477
and writing of the article.
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21
ACCEPTED MANUSCRIPT Acknowledgements:
479
Santanu Kaity is thankful to CSIR, New Delhi for financial support as CSIR-SRF [grant no.:
480
09/554(0029)/2011. EMR-I]. The authors are also thankful to CIF and the authority of BIT-
481
Mesra, Ranchi for providing necessary facilities for this work.
482
References:
483
[1] H. Kojima, K. Yoshihara, T. Sawad, H. Kondo, K. Sako, Extended release of large
484
amount of highly water soluble diltiazem hydrochloride by utilizing counter polymer in
485
polyethylene oxides (PEO)/polyethylene glycol (PEG) matrix tablets, Eur. J. Pharm.
486
Biopharm. 70 (2008) 556-562.
487
[2] A. Dashevsky, A. Mohamad, Development of pulsatile multiparticulate drug delivery
488
systemcoated with aqueous dispersion Aquacoat® ECD, Int. J Pharm. 318 (2006) 124-131.
489
[3] S. Ray, S. Banerjee, S. Maiti, B. Laha, S. Barik, B. Sa, U. K. Bhattacharyya, Novel
490
interpenetrating network microspheres of xanthan gum–poly(vinyl alcohol) for the delivery
491
of diclofenac sodium to the intestine- in vitro and in vivo evaluation, Drug Deliv. 17 (2010)
492
508-519.
493
[4] S. Mishra, R. Bajpai, R. Katare, A. K. Bajpai, Preparation, characterization and
494
microhardness study of semi interpenetrating polymer networks of poly(vinyl alcohol) and
495
crosslinked poly(acrylamide), J. Mater. Sci. - Mater. Med. 17 (2006) 1305-1313.
496
[5] T. R. Bhardwaj, M. Kanwar, R. Lal, A. Gupta, A. Natural gums and modified natural
497
gums as sustained-release carriers, Drug Dev. Ind. Pharm. 26 (2000) 1025-1038.
498
[6] V. Vijan, S. Kaity, S. Biswas, J. Isaac, A. Ghosh, Microwave assisted synthesis and
499
characterization of acrylamide grafted gellan, application in drug delivery, Carbohydr.
500
Polym. 90 (2012) 496-506.
AC C
EP
TE D
M AN U
SC
RI PT
478
22
ACCEPTED MANUSCRIPT [7] A. Lohani, G. Singh, S. S. Bhattacharya, A. Verma, Interpenetrating polymer networks as
502
innovative drug delivery systems, J. of Drug Del. 1 (2014) 1-11.
503
[8] A. G. Sullad, L. S. Manjeshwar, T. M. Aminabhavi, Novel semi-interpenetrating
504
microspheres of dextran-grafted-acrylamide and poly(vinyl alcohol) for controlled release of
505
abacavir sulfate, Ind. Eng. Chem. Res. 50 (2011) 11778-11784.
506
[9] S. A. Agnihotri, T. M. Aminabhavi, Development of novel interpenetrating network
507
gellan gum-poly(vinyl alcohol) hydrogel microspheres for the controlled release of
508
carvedilol, Drug Dev. Ind. Pharm. 31 (2005) 491-503.
509
[10] K. S. Soppimath, A. R. Kulkarni, T. M. Aminabhavi, Controlled release of
510
antihypertensive drug from the interpenetrating network poly(vinyl alcohol) – guar gum
511
hydrogel microspheres, J. Biomat. Sci- Polym. E. 11 (2000) 27-43.
512
[11] A. G. Sullad, L. S. Manjeshwar, T. M. Aminabhavi, Novel pH sensitive hydrogels
513
prepared from the blends of poly(vinyl alcohol) with acrylic acid-graft-guar gum matrixes for
514
isoniazid delivery, Ind. Eng. Chem. Res. 49 (2010) 7323-7329.
515
[12] M. C. Hassan, N. A. Peppas, Structure and applications of poly(vinyl alcohol) hydrogel
516
produced by conventional crosslinking or by freezing/thawing methods, Adv. Polym. Sci.
517
153 (2000) 37-62.
518
[13] S. Kaity, J. Isaac, A. Ghosh, Interpenetrating polymer network of locust bean gum-poly
519
(vinyl alcohol) for controlled release drug delivery, Carbohydr. Polym. 94 (2013) 456-467.
520
[14] P. B. Kajjari, L. S. Manjeshwar, T. M. Aminabhavi, Novel interpenetrating polymer
521
network hydrogel microspheres of chitosan and poly(acrylamide)-grafted-guar gum for
522
controlled release of ciprofloxacin, Ind. Eng. Chem. Res. 50 (2011) 13280-13287.
523
[15] K. S. Parvathy, N. S. Susheelamma, R. N. Tharanathan, A. K. Gaonkar, A simple non-
524
aqueous method for carboxymethylation of galactomanans, Carbohydr. Polym. 62 (2005)
525
137-141.
AC C
EP
TE D
M AN U
SC
RI PT
501
23
ACCEPTED MANUSCRIPT [16] D. R. Picout, S. B. Ross-Murphy, K. Jumel, S. E. Harding, Pressure cell assisted solution
527
characterization of polysaccharides. 2. locust bean gum and tara gum, Biomacromolecules. 3
528
(2002) 761-767.
529
[17] S. Kaity, A. Ghosh, Carboxymethylation of locust bean gum: application in
530
interpenetrating polymer network microspheres for controlled drug delivery, Ind. Eng. Chem.
531
Res. 52 (2013) 10033-10045.
532
[18] S. Kaity, J. Isaac, P. Mahesh, A. Bose, T. W. Wong, A. Ghosh, Microwave assisted
533
synthesis of acrylamide grafted locust bean gum and its application in drug delivery,
534
Carbohydr. Polym. 98 (2013) 1083-1094.
535
[19] A. Dubourg, R. F. Scamuffa, An experimental overview of a new vasoactive drug:
536
buflomedil HCl, Angiology.32 (1981) 663-675.
537
[20] C.S. Angadi, S. L. Manjeshwar, T. M. Aminabhai, Stearic acid-coated chitosan-based
538
interpenetrating polymer network microspheres: controlled release characteristics, Ind. Eng.
539
Chem. Res. 50 (2011) 4504-4514.
540
[21] B. F. Oliveira, M. H. A. Santana, M. I. Ré, Spray-dried chitosan microspheres cross-
541
linked with d, l-glyceraldehyde as a potential drug delivery system: preparation and
542
characterization, Braz. J. Chem. Eng. 22 (2005) 353-360.
543
[22] R. W. Korsemeyer, R. Gunny, E. Doelker, P. Buri, N. A. Peppas, Mechanism of solute
544
release from hydrophilic polymers, Int. J. Pharm. 15 (1983) 25-35.
545
[23] R. C. Mundargi, A. S. Patil, T. M. Aminabhavi, Evaluation of acrylamide grafted-
546
xanthan gum copolymer matrix tablets for oral controlled delivery of antihypertensive drugs,
547
Carbohydr. Polym. 69 (2007) 130-141.
548
[24] G. Andrade, E. F. Barbosa-Stancioli, A. A. P. Mansur, W. L. Vasconcelos, H. S.
549
Mansur, Small-angle x-ray scattering and FTIR characterization of nanostructured poly(vinyl
550
alcohol)/silicate hybrids for immunoassay applications, J. Mater. Sci. 43 (2008) 450-463.
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ACCEPTED MANUSCRIPT [25] H. S. Mansur, C. M. Sadahira, A. N. Souza, A. A. P. Mansur, FTIR spectroscopy
552
characterization of poly(vinyl alcohol) hydrogel with different hydrolysis degree and
553
chemically crosslinked with glutaraldehyde, Mater. Sci. Eng- C. 28 (2008) 539-548.
554
[26] K. H. Leong, L. Y. Chung, M. I. Noordin, K. Mohamad, M. Nishikawa, Y. Onuki, M.
555
Morishita, K. Takayama, Carboxymethylation of kappa-carrageenan for intestinal-targeted
556
delivery of bioactive macromolecules, Carbohydr. Polym. 83 (2011) 1507-1515.
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557
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560 561 562 563
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ACCEPTED MANUSCRIPT 1
Table 1. Representation of formulation code, different formulation variables, DEE, particle
2
size, PDI and equilibrium water uptake.
3
Gum:PVA
GA
Drug
DEE%
Particle
code
(Am-g-
(mL)
loading
(±SD, n=3)
size
LBG:PVA)
7 8 9
1:2
5.0
50
73.51±2.78
A2
1:1
2.5
25
51.32±1.94
A3
1:1
5.0
50
62.83±1.04
A4
1:1
5.0
25
A5
1:1
2.5
A6
1:2
A7
1:2
A8
1:2
A9
0:1
449.46
1.18
SC
A1
pH 6.8
235.13
317.28
1.03
281.55
354.17
608.76
1.12
252.49
332.10
59.74±1.82
551.91
1.32
247.36
328.97
50
55.29±1.43
766.06
1.00
293.41
361.58
2.5
50
68.11±2.15
519.36
1.09
255.27
328.85
2.5
25
65.68±1.55
476.12
0.82
248.53
326.77
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659.42
5.0
25
72.17±1.36
429.70
0.99
229.15
313.74
2.5
50
52.13±2.88
371.06
0.85
129.68
163.47
EP
6
pH 1.2
(µm)
AC C
5
Equilibrium water uptake (%)
[d(0.5)]
(%)
(w/w)
4
PDI
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Formulation
10 11
12 43
ACCEPTED MANUSCRIPT 13
Table 2.Representation of kinetic modelling of in vitro dissolution data Korsemeyer-Peppas Formulation
Zero
First
Higuchi
Hixson
code
order
order
kinetic
Crowell
A1
0.908
0.696
0.968
A2
0.906
0.699
A3
0.912
A4
R2
0.934
0.969
0.953
0.962
0.928
0.986
0.721
0.969
0.94
0.864
0.915
0.72
0.97
0.94
0.845
A5
0.929
0.742
0.972
0.947
0.86
A6
0.879
0.677
0.952
0.916
0.983
A7
0.864
0.664
0.938
0.902
1.032
A8
0.893
0.679
0.962
A9
0.863
0.651
0.938
15
T80%
0.391
0.219
0.353
0.959
0.195
0.282
0.956
0.151
0.263
0.961
0.151
0.263
0.942
0.239
0.385
0.931
0.262
0.413
SC
0.949
0.926
0.928
0.948
0.221
0.366
0.9
1.078
0.929
0.284
0.438
AC C
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14
0.24
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n
T50%
44
ACCEPTED MANUSCRIPT Figure captions: Figure 1: Pictorial representation of microspheres formation by emulsion crosslinking method. Figure 2: Three dimensional response surface plots: showing the effects of synthetic
Cumulative percentage drug release in dissolution study.
RI PT
condition on (a) DEE%(b) Particle size (c) Swelling in pH 1.2 (d) Swelling in pH 6.8 (e)
Figure 3: Proposed reaction mechanism of formation of acrylamide grafted locust bean gum
SC
and glutaraldehyde crosslinked acrylamide grafted locust bean gum poly(vinyl alcohol) hybridized network.
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Figure 4: FTIR spectra of PVA, physical mixture (PM), placebo, drug loaded formulation (DLF), buflomedil hydrochloride (BH) and acrylamide grafted locust bean gum (Am-gLBG). Figure 5: Solid state
13
C NMR spectra of Am-g-LBG, Am-g-LBG-PVA microspheres and
TE D
PVA.
Figure 6: DSC spectra of buflomedil hydrochloride (BH), PVA, Am-g-LBG, placebo microspheres and drug loaded microspheres.
EP
Figure 7: XRD patterns of BH, drug loaded microspheres and placebo microspheres. Figure 8: Scanning electron microscopy images of (a) Group of PVA microspheres (b) Am-
AC C
g-LBG-PVA network microspheres prepared by 2.5 mL GA (c) Am-g-LBG-PVA network microspheres prepared by 5.0 mL GA (d) Surface of Am-g-LBG-PVA network microspheres prepared by 5.0 mL GA (e-f) Cross sectional image of Am-g-LBG-PVA microspheres.. Figure 9: Particle size distribution of Am-g-LBG-PVA CR particles (A1-A9). Figure 10: In vitro dissolution characteristics of different batches of Am-g-LBG-PVA CR microspheres. 26
ACCEPTED MANUSCRIPT
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Am-g-LBG was added slowly and stirred for 3hr
0.5 mL 1 N Hcl was added and stirred for 30 min
Solution was cooled to room temperature
M AN U
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PVA dissolved in water (80⁰C)
Am-g-LBG-PVA blend was slowly emulsified with paraffin
Light liquid paraffin with Tween 80 mixed for 1 hr in a propeller stirrer
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Required amount of 25% GA was added and stirred for 3 h (500 RPM)
Particles vacuum dried in petridish and kept in desiccator until further use
Particles formed
Particles were filtered washed with acetone and 0.1 M glycine
SEM image of the particles
Figure 1: Pictorial representation of microspheres formation by emulsion crosslinking method. 27
ACCEPTED MANUSCRIPT
Design-Expert® Software Factor Coding: Actual DE% 73.51
(a)
51.32 X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde
75
Actual Factor C: % Drug loading = 0
70
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ACCEPTED MANUSCRIPT CH2 OH O H
OHH H OH H
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OH H
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CH2 OH O H H OH OH H H H
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Ceric ammoninum nitrate as redox initiator Microwave irradiation
H OH
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Acrylamide
O H
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OH H
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Hybridized network of acrylamide graf ted locu st bean gum and Poly(vinyl alcohol)
Figure 3: Proposed reaction mechanism of formation of acrylamide grafted locust bean gum and glutaraldehyde crosslinked acrylamide grafted locust bean gum-poly(vinyl alcohol) network. 31
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Figure 4: FTIR spectra of PVA, physical mixture (PM), placebo, drug loaded formulation (DLF), buflomedil hydrochloride (BH) and acrylamide grafted locust bean gum (Am-g-
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Figure 8: Scanning electron microscopy images of (a) Group of PVA microspheres (A9) (b) Am-g-LBG-PVA CR microspheres prepared by 2.5 mL GA (c) Am-g-LBG-PVA CR microspheres prepared by 5.0 mL GA (d) Surface of Am-g-LBG-PVA CR microspheres prepared by 5.0 mL GA (e-f) Cross sectional image of Am-g-LBG-PVA microspheres.
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Figure 10: In vitro dissolution characteristics of different batches of Am-g-LBG-PVA CR
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S1773-2247(16)30045-4
DOI:
10.1016/j.jddst.2016.02.005
Reference:
JDDST 169
To appear in:
Journal of Drug Delivery Science and Technology
Received Date: 18 December 2015 Revised Date:
2 February 2016
Accepted Date: 19 February 2016
Please cite this article as: S. Kaity, A. Ghosh, Facile preparation of acrylamide grafted locust bean gumpoly(vinyl alcohol) interpenetrating polymer network microspheres for controlled oral drug delivery, Journal of Drug Delivery Science and Technology (2016), doi: 10.1016/j.jddst.2016.02.005. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Am-g-LBG
Am-g-LBG-PVA blend
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Emulsion crosslinking
IPN microspheres
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For graphical abstract only
Controlled release of BH
ACCEPTED MANUSCRIPT ORIGINAL RESEARCH ARTICLE
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Facile preparation of acrylamide grafted locust bean gum-poly(vinyl alcohol)
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interpenetrating polymer network microspheres for controlled oral drug delivery
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Santanu Kaity and Animesh Ghosh*
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Department of Pharmaceutical Science and Technology, Birla Institute of Technology,
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Mesra, Ranchi- 835215, Jharkhand, India.
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* Corresponding author:
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Department of Pharmaceutical Sciences and Technology
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Birla Institute of Technology, Mesra
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Ranchi – 835215, Jhakhand, India.
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Tel.:+91-9470339587, Fax-+91-6512275290
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Email address: [email protected] (Animesh Ghosh)
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ACCEPTED MANUSCRIPT Abstract:
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Hybridization of natural and synthetic polymers is used to improve the physicochemical
25
stability, swelling and drug release pattern of the respective materials in biological condition.
26
In present study, a biodegradable, biocompatible and stable interpenetrating polymer network
27
(IPN) of acrylamide grafted locust bean gum (Am-g-LBG) and poly(vinyl alcohol) (PVA)
28
was developed by emulsion crosslinking method for spatial and temporal drug delivery. The
29
IPN microspheres were prepared with the help of glutaraldehyde as a crosslinker for
30
controlled oral delivery of buflomedil hydrochloride. The formulation parameters were
31
optimized in terms of different gum:PVA ratio, crosslinker amount and drug loading. The
32
microspheres were evaluated for their drug entrapment efficiency, particle size, swelling,
33
SEM, FTIR, NMR, DSC, XRD and in vitro drug release profile. The particles showed well
34
controlled release characteristics and continued to drug release following diffusion controlled
35
release pattern. The drug release was for prolong time without collapsing the particle matrix.
36
Thus, IPN microspheres based delivery system can be a better approach for controlled
37
delivery of highly water soluble drugs like buflomedil hydrochloride.
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Key words: Controlled release; Acrylamide grafted locust bean gum; Poly(vinyl alcohol);
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Buflomedil hydrochloride; Interpenetrating polymer network.
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ACCEPTED MANUSCRIPT 1. Introduction:
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The prime aim of controlled release drug delivery is “spatial placement” and “temporal
43
delivery”. Spatial placement refers to drug targeting to specific organs, tissue cells or even
44
sub-cellular compartments; whereas, temporal delivery refers to control the rate of drug
45
delivery to the target site.
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system can be a major advance towards delivering the drug molecules to their intended
47
destination. Multi-particulate delivery systems have gained special interest because of their
48
capability to meet the needs of spatial and temporal delivery of drug molecules with
49
minimum fluctuation of plasma drug concentration. [2]
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An interpenetrating polymer network (IPN) is a composite of two polymers, which obtained
51
when at least one polymer network is synthesized or cross-linked independently in the
52
immediate presence of the other.
53
improve mechanical properties and thermal stability.
54
polymer based network systems has extensively studied for drug delivery purpose as they are
55
biodegradable, biocompatible and can be tailored as intended.
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polymer combination of natural and synthetic origin has been found to be useful to control
57
the release of short half-lived drugs under physiological conditions. [7]
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Recently, a large number of IPN microspheres have been developed using different polymer
59
combinations for drug delivery purpose. Among them, Poly(vinyl alcohol) (PVA) based IPN
60
systems are extensively studied
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biocompatibility and desirable physical properties such as sufficient mechanical strength and
62
high degree of swelling in aqueous solution. [12] A combination of PVA with natural polymer
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may provide the system with better stability and improved mechanical strength to meet the
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major objectives of controlled release drug delivery.
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A strategically developed controlled release drug delivery
Chemical crosslinking between these polymers leads to [4]
In majority of the cases, the natural
[5, 6]
A judicially selected
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[1]
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[8-11]
due to its inherent non-toxicity, non-carcinogenicity,
3
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Various natural polymers have been explored for controlled-release microspheres
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development. Among them, guar gum, [10, 11] xanthan gum, [3] gellan gum, [9] locust bean gum,
67
[13]
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acrylamide grafted locust bean gum and PVA was selected as matrix for IPN based
69
microspheres development. To make a multi-particulate delivery system which will be able to
70
deliver the API for prolong time, the delivery device should have sufficient integrity during
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its GI residence. This hybridization was selected to make the matrix crosslinkable and to
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provide sufficient integrity to the particulate delivery device during its GI residence.
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Locust bean gum (LBG) is a high molecular weight branch polysaccharide and is extracted
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from the seeds of carob tree Ceratonia siliqua. It is a non-starch polysaccharides consisting
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of galactose and mannose in the ratio of 1:4 and hence they are known as galactomannan. [15]
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LBG is consists of (1,4)-linked β-D mannopyranose backbone with branch points from their
77
6-positions linked to α-D-galactose. The molecular weight of LBG ranges between 300,000
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and 1,200,000 Da. It is not easily soluble in water due to relatively hydrophobic nature of
79
mannan unit and requires heating to affect solvation. [16]
80
Recently, we have explored the efficiency of native LBG and carboxymethylated LBG
81
(CMLBG) with PVA as IPN controlled release drug delivery device.
82
observed poor entrapment efficiency of the particles. Moreover, in case of native LBG we
83
observed miscibility problem with aqueous PVA solution. Grafting of polyacrylamide onto
84
LBG can increase the aqueous solubility of resultant polymer.
85
grafted LBG and PVA may be able to overcome the problems observed in case of LBG-PVA
86
and CMLBG-PVA IPNs. So, in present study, IPN microspheres of acrylamide grafted locust
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bean gum (Am-g-LBG) and PVA was prepared for controlled oral delivery of a highly water-
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soluble drug, buflomedil hydrochloride (BH). BH is readily absorbed in the gastrointestinal
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tract and has a plasma half-life of approximately 2 to 3 h. The usual oral dose of BH is 300 to
[14]
has been reported till date. In present study, a novel combination of
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chitosan
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[13, 17]
In both cases we
IPN with acrylamide
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600 mg/day. Long-term use of BH in high doses can produce drug accumulation and drug
91
related toxicity.
92
BH, can reduce the dose and dose related side effects.
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The IPN particles of Am-g-LBG and PVA were developed by emulsion crosslinking method
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and the microspheres were evaluated for their drug entrapment efficiency, particle size,
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swelling, scanning electron microscopy (SEM), Fourier transform infrared spectroscopy
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(FTIR), nuclear magnetic resonance (NMR) spectroscopy, differential scanning colorimetry
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(DSC) and X-ray diffraction (XRD) profile. An in vitro drug release study [in both acidic
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media (pH 1.2) and phosphate buffer (pH 6.8)] and kinetic modelling was performed to
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understand the drug release mechanism.
Therefore, a controlled-release approach, such as IPN microspheres of
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[19]
2. Materials:
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Buflomedil hydrochloride was obtained as gift sample from Fresenius Kabi Oncology
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Limited (Kalyani, West Bengal, India). Locust bean gum and poly(vinyl alcohol) (PVA;
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average molecular weight 125000 Da) were purchased from HiMedia Laboratories Pvt. Ltd.
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(Mumbai, India). Light liquid paraffin (LLP; viscosity 25−80 mPa at 20°C), hydrochloric
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acid (HCl; 30%, ultra-pure) and acetone (Density = 0.789 to 0.791 g/mL) were obtained from
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Rankem India Pvt. Ltd. (Mumbai, India). Span 80 was procured from Pioneer In-Organics
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(Delhi, India). Glycine and glutaraldehyde (GA; 25%, v/v) were supplied by Merck India
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Ltd. (Mumbai, India). All the reagents were used without further purification. Water used
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was of Milli-Q grade.
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3. Methods:
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3.1. Synthesis of acrylamide grafted locust bean gum (Am-g-LBG)
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acrylamide grafted LBG. [18] In brief, 10 g of acrylamide (Am) was dissolved in 30 mL water
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and mixed with 120 mL aqueous dispersion of LBG (0.0083g/mL). 300 mg ceric ammonium
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nitrate (CAN) was dissolved in 30 mL of water and mixed with the Am-LBG mixture. The
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dispersion was irradiated by microwave (Laboratory scientific microwave system, Catalyst
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systems, India) at 480 W for 2.5 min. using alternate one minute heating and cooling cycle.
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The grafted gum was precipitated using acetone and washed with absolute and 30% aqueous
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ethanol. The grafted gum thus prepared was vacuum dried at 40⁰C to a constant weight and
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converted to fines for further use.
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3.2. Preparation of Am-g-LBG-PVA IPN microspheres
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Buflomedil hydrochloride (BH) entrapped IPN microspheres of PVA and Am-g-LBG were
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developed by water-in-oil (w/o) emulsion-crosslinking method (Figure 1). [14] Briefly, 20 mL
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of 2% (w/v) aqueous polymeric solution (total polymer amount was kept constant) was
125
prepared by dispersing varying amounts of Am-g-LBG in aqueous PVA solution. The
126
required amount of BH was added in the polymeric dispersion. The drug- polymer blend was
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slowly emulsified with light liquid paraffin (100 g) containing 1% (w/w) Tween-80 under
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constant mechanical stirring (IKA Labortechnik, Staufen, Germany) at 500 rpm. A milk
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white emulsion (w/o) was obtained. To this emulsion, GA (2.5 and 5 mL) containing 0.5 mL
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of 1 N HCl was added slowly and stirring was continued for 3 h. The crosslinked
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microspheres were then filtered and washed with acetone, 0.1 M glycine solution and water to
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remove excess amount of liquid paraffin, unreacted GA and surfactant, respectively.
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Complete removal of unreacted GA was confirmed by treating the filtrate with Fehling’s
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reagent. A negative result assured the absence of unreacted GA. Hardened microspheres were
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vacuum-dried at 40°C for 24 h and stored in desiccator until further use. The absence of
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crushed dried particles and treating it in similar way as said earlier.
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For the preparation of blank microspheres similar method was adopted except the addition of
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drug into the system. Detailed formulation variables are given in Table 1.
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Insert Table 1 here.
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Insert Figure 1 here.
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3.3. Full factorial design
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In the present study, two-level [high level (+1) and low level (−1)], three-factor, full factorial
145
design (8 batches) was used for the optimization of gum:PVA ratio, crosslinker and drug
146
loads (independent variables). The responses (dependent variables) selected for optimization
147
were drug entrapment efficiency, particle size, swelling and cumulative percentage drug
148
release in dissolution study. The results (Tables 1) of response generated using the
149
experimental designs were analysed by factorial models using Design Expert software
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(Version 7.0.0, Stat-Ease, Inc., Minneapolis). The 3D response plots are presented in Figure
151
2.
152
Insert Figure 2 here.
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3.4. Fourier transform infrared spectroscopy (FTIR)
154
The FTIR spectrums of Am-g-LBG, PVA, BH, drug-polymer physical mixture, blank
155
microspheres, and drug loaded microspheres were carried out by FTIR-8400S (Shimadzu,
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Japan) to confirm the formation of Am-g-LBG and compatibility of different ingredients of
157
the IPN formulations. A small amount of each material was mixed with potassium bromide
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(KBr) (1 %w/w sample content), taken into sample holder and scanned in the range of 600 to
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4000 cm-1.
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Solid state 13C NMR of Am-g-LBG, PVA and glutaraldehyde crosslinked blank formulation
162
was studied to confirm the formation of Am-g-LBG and glutaraldehyde crosslinked IPN
163
network. For solid state 13C NMR, approximately 300 mg of samples were inserted into the
164
ceramic rotor on a Bruker AMX 400 spectrometer. The spectrum was recorded at 75.5 MHz.
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3.6. Differential scanning calorimetry (DSC)
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DSC thermograms of Am-g-LBG, PVA, BH, blank formulation and drug loaded formulations
167
were obtained by using DSC-60 (Shimadzu, Japan). Each sample (3–7 mg) was accurately
168
weighed into a 40 µL aluminium pan in a hermetically sealed condition. The measurements
169
were conducted in nitrogen atmosphere between 30°C and 350°C at the heating rate of
170
10°C/min. The Am-g-LBG and the drug loaded formulations were heated in-situ up to 110⁰C
171
to make them moisture free. Then the samples were cooled to room temperature and reheated
172
up to 350⁰C.
173
3.7. Qualitative X-Ray diffractometry (XRD)
174
Grinded samples of blank IPN microspheres, drug loaded IPN microspheres, BH were
175
scanned from angular range of 10° to 60° 2θ, using an X-ray diffractometer (Bruker AXS D8
176
Advance, Germany, Configuration: Vertical, Theta/2 Theta geometry: X-ray Cu, wavelength
177
1.5406 A°, Detector: Si (Li) PSD. The diffractometer was run at a scanning speed of 2°/min
178
and a chart speed of 2°/2 cm per 2θ.
179
3.8. Scanning electron microscopy (SEM)
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The surface morphology and topography of Am-g-LBG-PVA IPN microspheres were
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evaluated by scanning electron microscope (JSM-6390LV, Jeol, Japan). Before examination,
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vacuum coated with gold palladium film (thickness 2 nm) by sputter coater (Edward S-150,
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U.K.) to make them electrically conductive. Representative sections were photographed for
185
evaluation.
186
3.9. Drug encapsulation efficiency (DEE)
187
IPN particles were crushed in mortar and pestle and a specified amount (10 mg) was taken
188
into 50 mL of phosphate buffer solution (pH 6.8), heated at 50°C for effective drug
189
extraction. After 24 h, the suspension was subjected for filtration and centrifugation for the
190
removal of polymeric debris. The supernatant was analysed with a spectrophotometer (UV-
191
1800, Shimadzu, Japan) at λmax of 282 nm. All samples were analysed in triplicate. The drug
192
entrapment efficiency (%) was calculated by using the following equation: [20]
193
Encapsulation efficiency (%) = (Actual drug content / Theoretical drug content) × 100
194
(1)
195
3.10. Swelling study
196
Equilibrium swelling study of IPN microspheres was done in different media. An accurately
197
weighed amount of microspheres (W1) was immersed in 50 mL buffer (pH 1.2 and pH 6.8)
198
and allowed to swell for 24 h at 37°C.The swollen microspheres was collected and the
199
adhered liquid droplets on the surface of the particles was removed carefully with tissue
200
paper and reweighed (W2) to an accuracy of ±0.01 mg on an electronic microbalance
201
(Mettler, model AT120, Greifensee, Switzerland). The swelling index was calculated by the
202
formula given below: [11]
203
Swelling index = [(W2-W1) / W1]× 100
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Where, W2 and W1 are the swollen and dry weights of the gum/microspheres, respectively.
Eq.
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Eq. (2)
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Particle size of IPN microspheres were determined by using a Mastersizer 2000 Ver.5.40
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(Malvern Instruments Ltd., UK) which allows sample measurement in the range of 20–2000
208
µm. The micro particles were dispersed in water and the size was measured using the laser
209
light scattering technique. Polydispersity index (PDI) was determined according to the
210
equation:
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Polydispersity index = [d(0.9) – d(0.1)]/d(0.5)
Eq. (3)
212
where, d(0.9), d(0.5) and d(0.1) are the particle diameters determined respectively at the 90th,
213
50th and 10th percentile of undersized particles. [21]
214
3.12. In vitro drug release and release kinetic study
215
In vitro drug release from the IPN microspheres were investigated in pH 1.2 for the initial 2
216
h, followed by phosphate buffer of pH 6.8. All the experiment was performed in triplicate in
217
a dissolution tester (Electro Lab, TDT-08L, India) equipped with eight baskets (glass jars) at
218
the stirring speed of 50 rpm. An accurately weighed quantity of each sample (equivalent to
219
100 mg BH) was placed in 900 mL of dissolution medium maintained at 37.5⁰C. At regular
220
intervals of time, sample aliquots were withdrawn and analysed using UV spectrophotometer
221
(UV-1800, Shimadzu, Japan) at the fixed λmax of 282 nm.
222
The release data were fitted in various empirical equations like Zero order (Qt = Kt), First
223
order (ln Qt= ln Q0-Kt ), Higuchi kinetic (Qt= Ktn), Hixson-Crowell (Q01/3- Qt1/3 = Kt) and the
224
power-law equation: Mt/M∞ = ktn, where Mt/M∞ is the fraction of drug release at time t, k is
225
the release rate constant, and n is the diffusion exponent that denotes the drug-release
226
mechanism. [22] A least squares regression method was used to determine the values of n and
227
k. Values of n = 0.43 or less indicate Fickian transport, whereas values of n of 0.43–0.85
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signifies the super case II transport mechanism.Q0 and Qt are amount of drug released at zero
230
and t time. K represents release rate constant.
231
4. Results and discussion:
232
The microwave assisted grafting method was used in present study to induce rapid energy to
233
the reaction system and to reduce the reaction time. The ceric ion from CAN generates free
234
radical sites on LBG backbone (Figure 3). LBG free radicals used to couple with acrylamide
235
by covalent linkage. The reaction is terminated by coupling of two free radicals.
236
details of synthetic parameters of IPN microspheres are given in Table 1. Acrylamide is an
237
excellent monomer which is freely soluble in water and can be mixed with hydrophilic gum
238
solution to make a homogenous blend. Thus it can easily attach with the adjacent gum
239
backbone by free radical polymerization thus reduce the chance of high amount of
240
homopolymer formation. Moreover acrylamide in low dose is non-toxic, easily excreted from
241
body and plasma half life is very less (2-2.5 h). The method of IPN particle preparation and
242
proposed reaction mechanism of IPN formation is shown in Figure 1 and Figure 3,
243
respectively. The general mechanism of matrix crosslinking with GA, a bi-functional
244
crosslinker, was through developing an acetal ring between the hydroxyl groups of Am-g-
245
LBG and PVA with the aldehyde groups of GA. This aided the formation of the IPN
246
microspheres in the emulsion phase. [14]
247
Insert Figure 3 here.
248
4.1. Fourier transform infrared spectroscopy (FTIR)
249
The FTIR spectral study of Am-g-LBG, buflomedil hydrochloride, PVA, physical mixture,
250
blank microspheres and optimized drug loaded microspheres (Figure 4) was performed to
[18]
The
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ACCEPTED MANUSCRIPT evaluate the compatibility of different formulation ingredients and to confirm the formation
252
of Am-g-LBG and GA crosslinked IPN matrix structure.
253
As presented in Figure 4, the Am-g-LBG showed the bands at 1683 and 1651 cm-1 were
254
attributed to amide-I (C–O stretching) and amide-II (N–H bending) conferred by Am. [23] The
255
peak at 2800–3566 cm−1 in Am-g-LBG was due to overlap of N–H stretching band of amide
256
group and O–H stretching band. A band at about 1454 cm−1 was due to the C–N stretching.
257
Peak at 1010 cm−1 was attributed to CH-O-CH2 group which occurs during grafting reaction
258
between OH group of C2 and π bond of acrylamide.
259
evidenced that LBG was successfully modified to Am-g-LBG.
260
For buflomedil hydrochloride major peaks were observed at about 2968 cm−1 for methoxy
261
CH stretching (CH3-O-). A small peak at about 1339 cm−1 was observed for aromatic C-N
262
stretching. Absorption band at 1701 cm-1 was of ketonic carbonyl group (Figure 4).
263
In case of PVA major peaks related to hydroxyl and acetate groups were present in FTIR
264
spectra. The large band observed between 3600 and 3200 cm−1 are linked to the O–H
265
stretching of the intermolecular and intramolecular hydrogen bonds. The vibrational band
266
observed between 2854 and 2944 cm−1 referred to the C–H stretching from alkyl groups and
267
the peaks between 1740–1716 cm−1 were due to the stretching C=O and C–O from acetate
268
group residues from PVA (Figure 4). A sharp peak obtained near 1456 cm-1 indicated the
269
bending vibration of CH2 groups. The intensity of the 1740– 1716 cm−1 strongly suggested
270
that it was less hydrolysed. [24]
271
The physical mixture showed the peaks of all components (BH, PVA and Am-g-LBG) in its
272
spectra without significant changes, indicating compatibility of the ingredients. The peak
273
intensities were observed to be reduced for all components due to the dilution effect.
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FTIR analysis of Am-g- LBG
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In the placebo Am-g-LBG-PVA IPN formulation, a considerable intensity reduction of the
275
O–H peaks from the PVA was noted, giving a possible indication of acetal bridge formation.
276
[25]
277
to ether linkage (C-O-C stretching) formed between the –OH group of PVA and Am-g-LBG
278
by the help of glutaraldehyde. [10] Peaks near about 1735 and 1650 cm −1 may be due to C=O
279
group of PVA acetate and amide-II (N–H bending) conferred by Am-g-LBG, respectively
280
(Figure 4). Thus, it can be said that Am-g-LBG and PVA was successfully crosslinked by GA
281
to form the network structure.
282
The drug loaded microspheres showed the additional peaks of BH in FTIR spectra than that
283
of placebo microspheres. Peaks at about 2925 cm−1 (methoxy CH stretching), 1338 cm−1
284
(aromatic C-N stretching) and 1702 cm-1 (ketonic carbonyl group) were due to BH (Figure 4).
285
No additional peaks were observed in the drug incorporated formulation than that of BH and
286
formulation components indicating that the ingredients itself and the process was compatible
287
for the preparation of BH loaded Am-g-LBG-PVA IPN microspheres.
288
Insert Figure 4 here.
289
4.2. Solid state 13C NMR spectroscopy
290
As per the earlier reports, the major peaks in the 13C NMR spectrum of LBG observed at δ =
291
62.0 ppm for the C-6 carbon of mannan unit, δ = 70-80 ppm for the signals of C-2, C-3 and
292
C-5 carbon atom, δ = 81.0 ppm for the C-4 mannan carbon atom and a sharp peak at δ =
293
102.7 ppm for C-1 mannan carbon atom. [13]
294
In the
295
CH2-CH-)n groups, formed due to Am polymerization, peak at δ=180.8 ppm for carbon atoms
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A small absorption peak at about 1250 cm −1 was observed in the spectrum which was due
13
C NMR spectrum of Am-g-LBG (Figure 5), the peak at δ=42.5 ppm was for (-CH-
13
ACCEPTED MANUSCRIPT of –CONH2 group. The NMR data strongly suggests that LBG was successfully converted to
297
Am-g-LBG.
298
The NMR spectrum of PVA consists of one broad peak at 45.8 ppm due to the methylene
299
carbon and a group of three peaks at δ = 62.8, 72.9, and 82.6 ppm from the oxymethine
300
carbon (Figure 5).
301
The
302
42.2 ppm due to the (-CH-CH2-CH-)n groups of acrylamide polymerization. The absorption
303
peak at δ = 61.3 ppm and 72.8 ppm are for PVA methine carbon. Peak at δ = 101.9 ppm is
304
due to the acetal carbon atom
305
group due to cross linking by glutaraldehyde proves the formation of IPN (Figure 5). The
306
broadened peak at δ = 177.4 ppm is for carbon atoms of –CONH2 group. Hence, the solid
307
state NMR spectra of the IPN particles showed a strong evidence of formation of
308
glutaraldehyde crosslinked IPN matrix of Am-g-LBG and PVA.
309
Insert Figure 5 here.
310
4.3. Differential scanning calorimetry (DSC)
311
From the DSC study it was observed that the Am-g-LBG showed its transition mid point
312
temperature (Tm) at about 238⁰C (Figure 6). It was almost similar as reported earlier. [18] PVA
313
showed its characteristic melting peak at about 192⁰C and a degradation peak was observed
314
at about 322⁰C (Figure 6). In case of pure BH, a sharp melting peak was observed at about
315
197⁰C which was matching with previous reports. [13] In case of placebo microspheres, peaks
316
due to individual components were hard to detect. However, a broad endothermic peak was
317
observed at about 288⁰C. This may be an indication of formation of a polymer composite
318
which degrades at a temperature other than the degradation points of individual basic
[17]
SC
C NMR spectrum of placebo Am-g-LBG-PVA IPN microspheres showed peak at δ=
which formed between the Am-g-LBG and PVA hydroxyl
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ACCEPTED MANUSCRIPT components. In drug loaded formulation, the endothermic peak at about 196⁰C was due to the
320
melting of entrapped BH (Figure 6). A broad endothermic peak was observed at about 278⁰C
321
which may be due to the degradation of the Am-g-LBG-PVA composite network structure.
322
Thus, from DSC study it can be said that a complex network structure was formed between
323
Am-g-LBG and PVA crosslinked by GA. Moreover, BH was successfully encapsulated in the
324
IPN polymer matrix.
325
Insert Figure 6 here.
326
4.4. Qualitative X-Ray diffractometry (XRD)
327
From the diffractogram of BH (Figure 7), it can be said that, it is highly crystalline in nature.
328
BH showed its characteristic peaks at 2θ of 6-50⁰. Sharp intense peak at about 2θ of 6⁰, 15⁰
329
and 21⁰ proves its crystalline nature. Drug loaded microspheres showed a broad peak at about
330
2θ of 20⁰. However, other peaks have disappeared in BH loaded microspheres assuring that
331
drug is molecularly dispersed in the polymer matrix. The peak intensity at 2θ of 20⁰ is higher
332
in drug loaded formulation than that of placebo confirms the presence of BH in IPN matrix.
333
Insert Figure 7 here.
334
4.5. Scanning electron microscopy (SEM)
335
The SEM image reveals surface morphology of the IPN particles and represented in Figure 8.
336
The particles which were prepared by PVA only (A9, Figure 8a) were having smooth surface
337
and well defined spherical structure. The particles prepared by Am-g-LBG and PVA in
338
combination with less amount of GA (Figure 8b) showed some pores on the surface.
339
However, the particles prepared with high amount of GA were appeared to be solid and there
340
was no pore on the surface (Figure 8c). This happened because of the higher crosslinking of
341
the polymer matrix. The surface appeared to be tough and showed evidence of network
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ACCEPTED MANUSCRIPT structure (Figure 8d). The cross sectional view of microspheres (Figure 8e and 8f) also
343
showed a strong evidence of the formation of well-defined polymer network structure.
344
Insert Figure 8 here.
345
4.6. Drug encapsulation efficiency (DEE)
346
The drug entrapment efficiency of Am-g-LBG-PVA IPN microspheres (Table 1) was
347
observed in the range of 51.32±1.94 (A2) to 73.51±2.78% (A1).This improvement in DEE
348
was due to the optimum miscibility of two phases and the highly branched structure of the
349
grafted gum which prevented the leaching of drug during the crosslinking stage. [18] The drug
350
entrapment capacity was observed to be dependent on the gum:PVA composition, crosslinker
351
and drug loads. A higher amount of Am-g-LBG (formulation code A2 - A5) led to reduced
352
DEE due to increased hydrophilicity of the system and inability of crosslinker to crosslink the
353
total system (Table 1). Similar findings were reported by Sullad et al. (2010).
354
increased amount of GA helped in higher drug entrapment due to the formation of rigid
355
polymer matrix (A1 and A6). Interestingly an increased drug loading showed least effect on
356
the DEE of the IPN microspheres (A1 and A8). This may be due to the saturation of the
357
matrix by the optimum drug concentration.
358
The three dimensional plot of the effects of different formulation variables on %DEE is
359
shown in Figure 2a. The mathematical relationship of DEE with the independent variables
360
was generated by MLRA and expressed as:
361
[11]
An
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DEE (%) = 63.58+6.29A+3.48B+1.35C
Eq. (4)
362
Where, A is gum:PVA ratio, B is glutaraldehyde amount and C is % drug loading. Here we
363
observed that all the independent variables were having positive impact on %DEE as was
364
observed experimentally. ANOVA analysis indicated that the model was significant (P < 16
ACCEPTED MANUSCRIPT 0.05) with R2 value 0.99. The adjusted (0.98) and predicted (0.96) R2 were reasonably in
366
good agreement.
367
4.7. Swelling study
368
The swelling of Am-g-LBG-PVA IPN microspheres (Table 1) was observed to be moderately
369
pH dependent. The extent of crosslinking played a major role in swelling of the microspheres.
370
Highly crosslinked particles (prepared with high amount of GA) showed less swelling (A1,
371
A3, A4 and A8) due to the absence of free hydrodynamic volume in their matrix. The
372
presence of higher amount of grafted gum in microspheres matrix resulted in higher swelling
373
(A2 in pH 1.2 and 6.8, respectively) (Table 1). This happened because of the hydrophilic
374
nature of the grafted gum. This postulation was further confirmed by the swelling
375
characteristics of microspheres having only PVA (A9) which showed least swelling in both
376
the media since it was devoid of grafted gum. The swelling of particles in acidic media (pH
377
1.2) was less in all cases than that of phosphate buffer (pH 6.8). Under pH 6.8, the presence
378
of ionisable groups in the component polymers which deprotonated and exhibited higher
379
swelling ratio due to the collective electrostatic repulsion forces between the ionized groups.
380
[26]
381
A slight increase in swelling was observed in case of formulation having higher drug loading
382
(A3 and A4). This was due to the increased hydrophilicity of the matrix in presence of highly
383
hydrophilic BH.
384
The effects of formulation variables on swelling as observed from MLRA are shown in
385
Figure 2c, 2d and expressed as:
386
Swelling% (pH 1.2) = 255.36 - 13.34A - 14.33B
387
Swelling % (pH 6.8) = 332.93 - 11.27A - 9.91B
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Eq. (5) Eq. (6)
ACCEPTED MANUSCRIPT Where, A is gum: PVA ratio and B is GA amount. ANOVA analysis indicated that the
389
factorial model was significant (P < 0.05) having R2 value of 0.91 and 0.92 for pH 1.2 and
390
pH 6.8, respectively. The adjusted (0.88 for both pH 1.2 and 6.8) and the predicted (0.78 and
391
0.79 for pH 1.2 and pH 6.8, respectively) R2 values were in reasonably good agreement. Here
392
both the gum: polymer ratio and GA showed negative effect and drug loading (%) showed
393
negligible influence on swelling as observed experimentally.
394
4.8. Particle size analysis
395
The arithmetic mean diameter of IPN particles varied from 371.06 µm to 766.06 µm (Figure
396
9, Table 1). In a fixed IPN blend composition, higher crosslinker amount resulted in
397
reduction of particle size (For A1 particle size is 449.46 µm, for A6 size is 519.36 µm). This
398
was due to the fact that as the amount of crosslinker was increased, the density of the polymer
399
matrix increased to a higher extent and reduced the internal void space.
400
The particle size was observed to be increased with the amount of Am-g-LBG (For A1
401
particle size was 449.46 µm, for A3 size was 608.76 µm) (Table 1). This can be explained on
402
the basis of hydrodynamic viscosity concept, i.e., with increased Am-g-LBG amount, the
403
interfacial viscosity of the polymer droplets in the emulsion was increased and resulted in the
404
formation of larger particles.
405
An increased drug loading (For A1 and A8 particle size was 429.70 µm and 449.46 µm
406
respectively) also resulted in the formation of bigger particles (Figure 9). The reason behind
407
this was, drug molecules might have hindered the inward shrinkage of the polymer matrix by
408
occupying the free volume spaces within the matrix. The polydispersity index of the Am-g-
409
LBG particles was less and it was in the range of 0.82 and 1.32 (Table 1). This result
410
indicates that the particles formed are of narrow size distribution range.
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ACCEPTED MANUSCRIPT 411
The effects of independent variables on the particle size are shown in Figure 2b. The
412
mathematical relationship is expressed as:
413
Particle size = 557.60 – 88.94A – 47.64B
414
Where, A is gum:PVA ratio and B is GA amount. ANOVA analysis indicated that the model
415
was significant (P < 0.05) with R2 value 0.87. The adjusted (0.83) and predicted (0.69) R2
416
were almost in good agreement. Here also we observed the negative effect of gum: PVA
417
ratio and GA on the size of IPN particles. It was in good agreement with experimental
418
observation.
419
Insert Figure 9 here.
420
4.9. In vitro drug release and release kinetic study
421
The cumulative percentage drug release vs. time plot of different batches of Am-g-LBG-PVA
422
IPN microspheres are presented in Figure 10. It was observed that the drug release from the
423
IPN microspheres were dependent upon major factors like crosslinker amount, polymeric
424
blend ratio and to less extent on the amount of drug loading.
425
Effect of crosslinker: In fixed formulating parameters, when the amount of crosslinker was
426
increased from 2.5 mL to 5 mL, the amount of drug release was decreased. In formulation A1
427
and A6 polymer composition (1:2) and drug loading (50%) was same but amount of
428
crosslinker was different. A1 showed less drug release (64%) than A6 (68%) (Figure 10).
429
This may be due to the higher crosslinking of the matrix which prevent solvent imbibition
430
and network erosion leading to high release retardant property.
431
Effect of gum:PVA blend ratio: When the blend ratio of IPN particles were changed from 1:2
432
to 1:1 in fixed crosslinker and drug loading percentage, the drug release increased from 64%
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ACCEPTED MANUSCRIPT (A1) to 79% (A3) and 68% (A6) to 87% (A2). This was due to the hydrophilic nature of the
434
grafted gum which interacted with media to swell and erode in a faster rate and helped in
435
faster drug release. Particles composed of only PVA (A9) showed 74% drug release in 12 h
436
(Figure 10).
437
Effect of drug loading: Formulations, having different drug loading in a fixed gum: PVA
438
ratio and crosslinker amount, showed different extent of drug release. For example, A2 (25%
439
drug loading, 87% drug release) showed retarded drug release property than A5 (50% drug
440
loading, 93% drug release) (Figure 10) though other parameters for both the formulations
441
were same. It may be due to the reason that, concentration gradient, the driving force, will be
442
high in high drug load formulations and promoted faster drug release. Moreover, low drug
443
load matrix would have a greater gum and polymer fraction to act as the barrier to drug
444
release.
445
The effect of formulation variables on CPR is shown in figure 2e and the mathematical
446
relation is expressed as:
447
CPR = 75.90 - 9.08A – 4.18B
448
Where, A is gum:PVA ratio and B is amount of GA. ANOVA analysis indicated that the
449
model was significant (P < 0.05) with R2 value 0.95. The adjusted (0.93) and predicted (0.88)
450
R2 were in good agreement. The effect of gum: polymer ratio and GA was similar to that of
451
experimental evidence.
452
After generating the model polynomial equations to relate the dependent and independent
453
variables, the best optimized amount of independent variables was finalized in terms of
454
maximum gum: PVA ratio, minimum amount of crosslinker and maximum drug loading to
455
achieve the dependent variables in terms of maximize DEE%, particle size in range,
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20
ACCEPTED MANUSCRIPT maximize swelling and minimum CPR. The software generated solution was in good
457
agreement with batch A6.The optimized Am-g-LBG-PVA IPN particles showed 68.08% drug
458
release at 12 h.
459
Release kinetic: The invitro release data were fitted in different empirical equations and
460
presented in Table 2. It was observed that the best fit was with Higuchi release kinetic,
461
suggesting that the release of drug molecules from IPN matrix was diffusion controlled. The
462
drug release data were also fitted with the Power law equation and the values of n varied
463
from 0.845 to 1.078. For A4 drug release was non Fickian and for the rest the release pattern
464
followed super case II transport mechanism.
465
Insert Figure 10 here.
466
Insert Table 2 here.
467
5. Conclusion:
468
In present study Am-g-LBG-PVA IPN microspheres were successfully prepared by emulsion
469
crosslinking method by using glutaraldehyde as a crosslinker. Among various formulations
470
the A6 batch was the optimized formulation. The particles were spherical with narrow size
471
distribution. The particle showed promising controlled release property with moderate pH
472
sensitivity. This type of polymeric composites may be fruitful as a promising biomaterial to
473
solve the major loop holes of controlled release of highly water soluble drugs with short half
474
life.
475
Conflict of interest:
476
The authors report no conflicts of interest. The authors alone are responsible for the content
477
and writing of the article.
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ACCEPTED MANUSCRIPT Acknowledgements:
479
Santanu Kaity is thankful to CSIR, New Delhi for financial support as CSIR-SRF [grant no.:
480
09/554(0029)/2011. EMR-I]. The authors are also thankful to CIF and the authority of BIT-
481
Mesra, Ranchi for providing necessary facilities for this work.
482
References:
483
[1] H. Kojima, K. Yoshihara, T. Sawad, H. Kondo, K. Sako, Extended release of large
484
amount of highly water soluble diltiazem hydrochloride by utilizing counter polymer in
485
polyethylene oxides (PEO)/polyethylene glycol (PEG) matrix tablets, Eur. J. Pharm.
486
Biopharm. 70 (2008) 556-562.
487
[2] A. Dashevsky, A. Mohamad, Development of pulsatile multiparticulate drug delivery
488
systemcoated with aqueous dispersion Aquacoat® ECD, Int. J Pharm. 318 (2006) 124-131.
489
[3] S. Ray, S. Banerjee, S. Maiti, B. Laha, S. Barik, B. Sa, U. K. Bhattacharyya, Novel
490
interpenetrating network microspheres of xanthan gum–poly(vinyl alcohol) for the delivery
491
of diclofenac sodium to the intestine- in vitro and in vivo evaluation, Drug Deliv. 17 (2010)
492
508-519.
493
[4] S. Mishra, R. Bajpai, R. Katare, A. K. Bajpai, Preparation, characterization and
494
microhardness study of semi interpenetrating polymer networks of poly(vinyl alcohol) and
495
crosslinked poly(acrylamide), J. Mater. Sci. - Mater. Med. 17 (2006) 1305-1313.
496
[5] T. R. Bhardwaj, M. Kanwar, R. Lal, A. Gupta, A. Natural gums and modified natural
497
gums as sustained-release carriers, Drug Dev. Ind. Pharm. 26 (2000) 1025-1038.
498
[6] V. Vijan, S. Kaity, S. Biswas, J. Isaac, A. Ghosh, Microwave assisted synthesis and
499
characterization of acrylamide grafted gellan, application in drug delivery, Carbohydr.
500
Polym. 90 (2012) 496-506.
AC C
EP
TE D
M AN U
SC
RI PT
478
22
ACCEPTED MANUSCRIPT [7] A. Lohani, G. Singh, S. S. Bhattacharya, A. Verma, Interpenetrating polymer networks as
502
innovative drug delivery systems, J. of Drug Del. 1 (2014) 1-11.
503
[8] A. G. Sullad, L. S. Manjeshwar, T. M. Aminabhavi, Novel semi-interpenetrating
504
microspheres of dextran-grafted-acrylamide and poly(vinyl alcohol) for controlled release of
505
abacavir sulfate, Ind. Eng. Chem. Res. 50 (2011) 11778-11784.
506
[9] S. A. Agnihotri, T. M. Aminabhavi, Development of novel interpenetrating network
507
gellan gum-poly(vinyl alcohol) hydrogel microspheres for the controlled release of
508
carvedilol, Drug Dev. Ind. Pharm. 31 (2005) 491-503.
509
[10] K. S. Soppimath, A. R. Kulkarni, T. M. Aminabhavi, Controlled release of
510
antihypertensive drug from the interpenetrating network poly(vinyl alcohol) – guar gum
511
hydrogel microspheres, J. Biomat. Sci- Polym. E. 11 (2000) 27-43.
512
[11] A. G. Sullad, L. S. Manjeshwar, T. M. Aminabhavi, Novel pH sensitive hydrogels
513
prepared from the blends of poly(vinyl alcohol) with acrylic acid-graft-guar gum matrixes for
514
isoniazid delivery, Ind. Eng. Chem. Res. 49 (2010) 7323-7329.
515
[12] M. C. Hassan, N. A. Peppas, Structure and applications of poly(vinyl alcohol) hydrogel
516
produced by conventional crosslinking or by freezing/thawing methods, Adv. Polym. Sci.
517
153 (2000) 37-62.
518
[13] S. Kaity, J. Isaac, A. Ghosh, Interpenetrating polymer network of locust bean gum-poly
519
(vinyl alcohol) for controlled release drug delivery, Carbohydr. Polym. 94 (2013) 456-467.
520
[14] P. B. Kajjari, L. S. Manjeshwar, T. M. Aminabhavi, Novel interpenetrating polymer
521
network hydrogel microspheres of chitosan and poly(acrylamide)-grafted-guar gum for
522
controlled release of ciprofloxacin, Ind. Eng. Chem. Res. 50 (2011) 13280-13287.
523
[15] K. S. Parvathy, N. S. Susheelamma, R. N. Tharanathan, A. K. Gaonkar, A simple non-
524
aqueous method for carboxymethylation of galactomanans, Carbohydr. Polym. 62 (2005)
525
137-141.
AC C
EP
TE D
M AN U
SC
RI PT
501
23
ACCEPTED MANUSCRIPT [16] D. R. Picout, S. B. Ross-Murphy, K. Jumel, S. E. Harding, Pressure cell assisted solution
527
characterization of polysaccharides. 2. locust bean gum and tara gum, Biomacromolecules. 3
528
(2002) 761-767.
529
[17] S. Kaity, A. Ghosh, Carboxymethylation of locust bean gum: application in
530
interpenetrating polymer network microspheres for controlled drug delivery, Ind. Eng. Chem.
531
Res. 52 (2013) 10033-10045.
532
[18] S. Kaity, J. Isaac, P. Mahesh, A. Bose, T. W. Wong, A. Ghosh, Microwave assisted
533
synthesis of acrylamide grafted locust bean gum and its application in drug delivery,
534
Carbohydr. Polym. 98 (2013) 1083-1094.
535
[19] A. Dubourg, R. F. Scamuffa, An experimental overview of a new vasoactive drug:
536
buflomedil HCl, Angiology.32 (1981) 663-675.
537
[20] C.S. Angadi, S. L. Manjeshwar, T. M. Aminabhai, Stearic acid-coated chitosan-based
538
interpenetrating polymer network microspheres: controlled release characteristics, Ind. Eng.
539
Chem. Res. 50 (2011) 4504-4514.
540
[21] B. F. Oliveira, M. H. A. Santana, M. I. Ré, Spray-dried chitosan microspheres cross-
541
linked with d, l-glyceraldehyde as a potential drug delivery system: preparation and
542
characterization, Braz. J. Chem. Eng. 22 (2005) 353-360.
543
[22] R. W. Korsemeyer, R. Gunny, E. Doelker, P. Buri, N. A. Peppas, Mechanism of solute
544
release from hydrophilic polymers, Int. J. Pharm. 15 (1983) 25-35.
545
[23] R. C. Mundargi, A. S. Patil, T. M. Aminabhavi, Evaluation of acrylamide grafted-
546
xanthan gum copolymer matrix tablets for oral controlled delivery of antihypertensive drugs,
547
Carbohydr. Polym. 69 (2007) 130-141.
548
[24] G. Andrade, E. F. Barbosa-Stancioli, A. A. P. Mansur, W. L. Vasconcelos, H. S.
549
Mansur, Small-angle x-ray scattering and FTIR characterization of nanostructured poly(vinyl
550
alcohol)/silicate hybrids for immunoassay applications, J. Mater. Sci. 43 (2008) 450-463.
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ACCEPTED MANUSCRIPT [25] H. S. Mansur, C. M. Sadahira, A. N. Souza, A. A. P. Mansur, FTIR spectroscopy
552
characterization of poly(vinyl alcohol) hydrogel with different hydrolysis degree and
553
chemically crosslinked with glutaraldehyde, Mater. Sci. Eng- C. 28 (2008) 539-548.
554
[26] K. H. Leong, L. Y. Chung, M. I. Noordin, K. Mohamad, M. Nishikawa, Y. Onuki, M.
555
Morishita, K. Takayama, Carboxymethylation of kappa-carrageenan for intestinal-targeted
556
delivery of bioactive macromolecules, Carbohydr. Polym. 83 (2011) 1507-1515.
RI PT
551
557
SC
558 559
M AN U
560 561 562 563
EP AC C
565
TE D
564
25
ACCEPTED MANUSCRIPT 1
Table 1. Representation of formulation code, different formulation variables, DEE, particle
2
size, PDI and equilibrium water uptake.
3
Gum:PVA
GA
Drug
DEE%
Particle
code
(Am-g-
(mL)
loading
(±SD, n=3)
size
LBG:PVA)
7 8 9
1:2
5.0
50
73.51±2.78
A2
1:1
2.5
25
51.32±1.94
A3
1:1
5.0
50
62.83±1.04
A4
1:1
5.0
25
A5
1:1
2.5
A6
1:2
A7
1:2
A8
1:2
A9
0:1
449.46
1.18
SC
A1
pH 6.8
235.13
317.28
1.03
281.55
354.17
608.76
1.12
252.49
332.10
59.74±1.82
551.91
1.32
247.36
328.97
50
55.29±1.43
766.06
1.00
293.41
361.58
2.5
50
68.11±2.15
519.36
1.09
255.27
328.85
2.5
25
65.68±1.55
476.12
0.82
248.53
326.77
TE D
M AN U
659.42
5.0
25
72.17±1.36
429.70
0.99
229.15
313.74
2.5
50
52.13±2.88
371.06
0.85
129.68
163.47
EP
6
pH 1.2
(µm)
AC C
5
Equilibrium water uptake (%)
[d(0.5)]
(%)
(w/w)
4
PDI
RI PT
Formulation
10 11
12 43
ACCEPTED MANUSCRIPT 13
Table 2.Representation of kinetic modelling of in vitro dissolution data Korsemeyer-Peppas Formulation
Zero
First
Higuchi
Hixson
code
order
order
kinetic
Crowell
A1
0.908
0.696
0.968
A2
0.906
0.699
A3
0.912
A4
R2
0.934
0.969
0.953
0.962
0.928
0.986
0.721
0.969
0.94
0.864
0.915
0.72
0.97
0.94
0.845
A5
0.929
0.742
0.972
0.947
0.86
A6
0.879
0.677
0.952
0.916
0.983
A7
0.864
0.664
0.938
0.902
1.032
A8
0.893
0.679
0.962
A9
0.863
0.651
0.938
15
T80%
0.391
0.219
0.353
0.959
0.195
0.282
0.956
0.151
0.263
0.961
0.151
0.263
0.942
0.239
0.385
0.931
0.262
0.413
SC
0.949
0.926
0.928
0.948
0.221
0.366
0.9
1.078
0.929
0.284
0.438
AC C
EP
TE D
16
M AN U
14
0.24
RI PT
n
T50%
44
ACCEPTED MANUSCRIPT Figure captions: Figure 1: Pictorial representation of microspheres formation by emulsion crosslinking method. Figure 2: Three dimensional response surface plots: showing the effects of synthetic
Cumulative percentage drug release in dissolution study.
RI PT
condition on (a) DEE%(b) Particle size (c) Swelling in pH 1.2 (d) Swelling in pH 6.8 (e)
Figure 3: Proposed reaction mechanism of formation of acrylamide grafted locust bean gum
SC
and glutaraldehyde crosslinked acrylamide grafted locust bean gum poly(vinyl alcohol) hybridized network.
M AN U
Figure 4: FTIR spectra of PVA, physical mixture (PM), placebo, drug loaded formulation (DLF), buflomedil hydrochloride (BH) and acrylamide grafted locust bean gum (Am-gLBG). Figure 5: Solid state
13
C NMR spectra of Am-g-LBG, Am-g-LBG-PVA microspheres and
TE D
PVA.
Figure 6: DSC spectra of buflomedil hydrochloride (BH), PVA, Am-g-LBG, placebo microspheres and drug loaded microspheres.
EP
Figure 7: XRD patterns of BH, drug loaded microspheres and placebo microspheres. Figure 8: Scanning electron microscopy images of (a) Group of PVA microspheres (b) Am-
AC C
g-LBG-PVA network microspheres prepared by 2.5 mL GA (c) Am-g-LBG-PVA network microspheres prepared by 5.0 mL GA (d) Surface of Am-g-LBG-PVA network microspheres prepared by 5.0 mL GA (e-f) Cross sectional image of Am-g-LBG-PVA microspheres.. Figure 9: Particle size distribution of Am-g-LBG-PVA CR particles (A1-A9). Figure 10: In vitro dissolution characteristics of different batches of Am-g-LBG-PVA CR microspheres. 26
ACCEPTED MANUSCRIPT
RI PT
Am-g-LBG was added slowly and stirred for 3hr
0.5 mL 1 N Hcl was added and stirred for 30 min
Solution was cooled to room temperature
M AN U
SC
PVA dissolved in water (80⁰C)
Am-g-LBG-PVA blend was slowly emulsified with paraffin
Light liquid paraffin with Tween 80 mixed for 1 hr in a propeller stirrer
AC C
EP
TE D
Required amount of 25% GA was added and stirred for 3 h (500 RPM)
Particles vacuum dried in petridish and kept in desiccator until further use
Particles formed
Particles were filtered washed with acetone and 0.1 M glycine
SEM image of the particles
Figure 1: Pictorial representation of microspheres formation by emulsion crosslinking method. 27
ACCEPTED MANUSCRIPT
Design-Expert® Software Factor Coding: Actual DE% 73.51
(a)
51.32 X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde
75
Actual Factor C: % Drug loading = 0
70
RI PT
65
DE%
60 55 50
1
0.5 0
SC
1
0.5
0
-0.5
B: Glutaraldehyde
-0.5
A: Gum Polymer ratio
-1
M AN U
-1
Design-Expert® Software Factor Coding: Actual PS 766.06 429.7
700
(b)
600
PS
Actual Factor C: % Drug loading = 0
TE D
800
X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde
500
AC C
EP
400
1
0.5
0
B: Glutaraldehyde
1 0.5
-0.5 0 -0.5 -1
-1
A: Gum Polymer ratio
28
ACCEPTED MANUSCRIPT Design-Expert® Software Factor Coding: Actual Swelling(1.2) 293.41 229.15
(c)
X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde
300
Actual Factor C: % Drug loading = 0
260 240
RI PT
Swelling(1.2)
280
220
1
1
0.5
0.5
0
B: Glutaraldehyde
-0.5
SC
0
-0.5
A: Gum Polymer ratio
X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde
370
360
350
340
330
AC C
EP
Swelling(6.8)
Actual Factor C: % Drug loading = 0
(d)
TE D
Design-Expert® Software Factor Coding: Actual Swelling(6.8) 361.58 313.74
-1
M AN U
-1
320
310
1 1 0.5
0.5 0
0 -0.5
B: Glutaraldehyde
-0.5 -1
29
-1
A: Gum Polymer ratio
ACCEPTED MANUSCRIPT Design-Expert® Software Factor Coding: Actual CPR 93.16
(e)
59.99 X1 = A: Gum Polymer ratio X2 = B: Glutaraldehyde Actual Factor C: % Drug loading = 0
100 90
70
RI PT
CPR
80
60 50
1
1
0.5
0.5
0
0 -0.5
-0.5
SC
B: Glutaraldehyde
A: Gum Polymer ratio
-1
M AN U
-1
Figure 2: Three dimensional response surface plots: showing the effects of synthetic condition on (a) DEE%(b) Particle size (c) Swelling in pH 1.2 (d) Swelling in pH 6.8 (e)
AC C
EP
TE D
Cumulative percentage drug release in dissolution study.
30
ACCEPTED MANUSCRIPT CH2 OH O H
OHH H OH H
H O OH H2 C
H O
H H OH OH H
H H OH
O OH H
OH H
H
O
O CH2 OH
H
CH2 OH O H H OH OH H H H
H
O
H OH
OH H H
O CH2 OH
RI PT
Locu st bean gum
Ceric ammoninum nitrate as redox initiator Microwave irradiation
H OH
H OH
H
Acrylamide
O H
CH 2 O
H H OH OH H
OH H
H
CH2 H H OH
H H OH
O OH H
O
O CH2 O CH2
H
C
H
SC
OHH
OH O H
OH O
OH H H
H
H
CONH2
Initiation
H
O
OH H H
OH
OH
H
H
OH
n OH
H
H
CH2 O
H H OH
H
H
OH H
H
OH O
O
H
CH 2 O CH 2 C CH 2
CONH2
C
CONH2
C
CONH 2
CH C
OH
H H
O
CONH2
O
O
H
H
H
H
O
H OH
OH H H
O
H CH 2
CH O
CH2 CONH2
CH2 C
H
O
AC C
CH
H OH O
(CH2 )3
CH2
H
OH H
Elongation and termination
O
CH2
EP
H
CH2
H
O
OH
OH H
Gluteraldehyde Hydrochloric acid
Polyvinyl alcoh ol
O
H
OCH(CH2)3 CHO
TE D
CH2
H
H2 C
Acrylamide grafted locust bean gum CH2CH
H
O
M AN U
CH2
CONH 2
CH2 H
CH2 CH
C
CONH2
H 2C
n H
C
CONH2
CH H
C
CONH2
Hybridized network of acrylamide graf ted locu st bean gum and Poly(vinyl alcohol)
Figure 3: Proposed reaction mechanism of formation of acrylamide grafted locust bean gum and glutaraldehyde crosslinked acrylamide grafted locust bean gum-poly(vinyl alcohol) network. 31
TE D
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
Figure 4: FTIR spectra of PVA, physical mixture (PM), placebo, drug loaded formulation (DLF), buflomedil hydrochloride (BH) and acrylamide grafted locust bean gum (Am-g-
AC C
EP
LBG).
32
M AN U
SC
RI PT
ACCEPTED MANUSCRIPT
AC C
EP
TE D
Figure 5: Solid state 13C NMR spectra of Am-g-LBG, Am-g-LBG-PVA network and PVA.
33
M AN U
SC
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ACCEPTED MANUSCRIPT
TE D
Figure 6: DSC spectra of buflomedil hydrochloride (BH), PVA, Am-g-LBG, placebo
AC C
EP
microspheres and drug loaded microspheres.
34
M AN U
SC
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ACCEPTED MANUSCRIPT
AC C
EP
TE D
Figure 7: XRD patterns of BH, drug loaded microspheres and placebo microspheres.
35
AC C
EP
TE D
M AN U
SC
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ACCEPTED MANUSCRIPT
Figure 8: Scanning electron microscopy images of (a) Group of PVA microspheres (A9) (b) Am-g-LBG-PVA CR microspheres prepared by 2.5 mL GA (c) Am-g-LBG-PVA CR microspheres prepared by 5.0 mL GA (d) Surface of Am-g-LBG-PVA CR microspheres prepared by 5.0 mL GA (e-f) Cross sectional image of Am-g-LBG-PVA microspheres.
36
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
A1
37
A2
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
A3
38
A4
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
RI PT
A5
39
A6
ACCEPTED MANUSCRIPT
AC C
EP
TE D
M AN U
SC
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A7
40
A8
ACCEPTED MANUSCRIPT
M AN U
SC
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A9
AC C
EP
TE D
Figure 9: Particle size distribution of Am-g-LBG-PVA hybridized particles (A1-A9).
41
M AN U
SC
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Figure 10: In vitro dissolution characteristics of different batches of Am-g-LBG-PVA CR
AC C
EP
TE D
microspheres.
42