The effect of MgCl2.6H2O and NaF on properties of Chitosan / HA-Al2O3 Scaffold
Fateme Mirjalili
1
(
Department of material engineering,faculty of engineering,Islamic azad university Maybod beranch,Iran
)
esmail salahi
2
(
Energy and Environmental Department, Materials and Energy Research Center, P.O. Box 31787-316, Karaj, Iran
)
Ali kaffashiyan
3
(
2Department of Material Engineering, Yazd Branch, Islamic Azad University, Yazd, Iran
)
Keywords: Alumina, scaffold, HA, nano, Chitosan/ HA- Al2O3 scaffold,
Abstract :
The HA- Al2O3 nano composite was produced by precipitation method. In the first study,the effect of MgCl2.6H2O and NaF additives on HA-Al2O3 nano-composite powder were studied and the second, chitosan / HA- Al2O3 scaffold was prepared by freeze casting method. The phase and microstructure and morphology analysis of nano composite and scaffold were performed by XRD, FT-IR, FESEM and TEM. X-ray diffraction test results along with infrared spectroscopy indicated that, the HA- Al2O3 nano composite without impurities were produced. TEM result showed that, the produced nano cmposite particle sizes were reported between 30-50 nm.Moreover, the porosity percentages of scaffold without additive was about 56% and with NaF as an additive was about 63 %, however, the scaffold with MgCl2.6H2O additive with 70% porosity had the highest porosity percentage. The compressive strength of the SFA scaffold exhibited a two-fold strength compared to the SMA scaffold, which indicated the improved mechanical compatibility of the SFA scaffold.
The effect of MgCl2.6H2O and NaF on properties of Chitosan / HA-Al2O3 Scaffold
The HA- Al2O3 nano composite was produced by precipitation method. In the first study,
the effect of MgCl2.6H2O and NaF additives on HA-Al2O3 nano-composite powder were studied and the second, chitosan / HA- Al2O3 scaffold was prepared by freeze casting method. The phase and microstructure and morphology analysis of nano composite and scaffold were performed by XRD, FT-IR, FESEM and TEM. X-ray diffraction test results along with infrared spectroscopy indicated that, the HA- Al2O3 nano composite without impurities were produced. TEM result showed that, the produced nano cmposite particle sizes were reported between 30-50 nm.
Moreover, the porosity percentages of scaffold without additive was about 56% and with NaF as an additive was about 63 %, however, the scaffold with MgCl2.6H2O additive with 70% porosity had the highest porosity percentage. The compressive strength of the SFA scaffold exhibited a two-fold strength compared to the SMA scaffold, which indicated the improved mechanical compatibility of the SFA scaffold.
Keywords: Nano, Scaffold, HA, Alumina, Chitosan/ HA- Al2O3 scaffold
1. Introduction:
Bone regeneration is a complex cascade of biological events which controlled by numerous molecules and provides signals at local injury sites allowing progenitors and inflammatory cells to migrate and trigger healing processes. Conventional tissue engineering strategies utilize combination of cells, biodegradable scaffolds and systemic administration of bioactive molecules to promote natural processes of tissue regeneration and development [1-3]. A number of strategies for controlled biomolecule delivery from scaffolds have been developed for bone tissue engineering. One of the most common methods to achieve controlled and localized release of biomolecules is to incorporate them within biomaterials during the phase of scaffold fabrication [4]. According to this approach, the properties of the scaffolds, such as pore size and crosslinking density can control the biomolecule release rate by diffusion. In addition, the rate of scaffold degradation affects the biomolecule release rate over a prolonged time period [5-6]. Implantation of bone auto grafts or allografts is a simple strategy to heal large bone defects [7]. However, there are some drawbacks of these strategies which limit their widespread usage, such as extended surgical time and donor site morbidity for auto graft and adverse immune response and pathogen disease transmission for allograft. These problems have guided researchers for the development of bone substitute materials [8–12]. As the most promising bone substitute materials, calcium phosphate (CP) compounds have been widely used clinically due to their similarity to hard tissues [13].
Among different CP ceramics hydroxyapatite (HA) and tri-calcium phosphate (TCP), or combinations of these two materials (biphasic ceramics) have gained special attentions for a wide range of applications such as maxillofacial reconstruction [14-16], orbital implants [17], spine fusion [18] and repair of bone defects [19]. These materials have been clinically used in dense, granular and porous forms [20–22]. Hydroxyapatite is calcium phosphate nearest to bone mineral and the most thermodynamically stable phase in the body [2, 23]. Calcium phosphates, such as hydroxyapatite for their biocompatibility and similarity to the mineral components of bones and teeth are good replacements for parts of the body which are damaged [1, 24]. Hydroxyapatite increases the capability of bone growth and forms a strong chemical bond with bone tissue when the bone tissue grow in the surface layer of this ceramic [3,25]. Nonetheless it is a brittle material which leads to low mechanical failure and limits its application in a position under the load. Therefore, it is important to add a secondary phase to improve the strength and mechanical properties of hydroxyapatite. The most important materials such as alumina, zirconia, titania and organic glass can be used as the reinforcing components [4, 26]. Due to its unique thermal, mechanical, and chemical properties, alumina is applied widely in the strong materials, composites and reinforcing materials. Alumina as the engineering ceramic based on its high mechanical properties and biocompatible properties is used as bone and dental fittings [5, 27]. Moreover, its application in biology increases owing to hardness, high strength against fatigue and resistance to corrosion [28]. NaF and MgCl2 .6H2O nanocrystalline ceramics have biocompatibility and bioactivity and similarities to bone mineral parts in many bone marrow engineering scaffolds, metal surface coatings, and drug delivery and delivery [29].
The replacement of various ions such as sodium (Na), magnesium (Mg), fluorine (F), chlorine (Cl), aluminum (Al) improves chemical composition and structure of apatite. Ion substitution in the apatite structure not only leads to improving the biocompatibility, bioactivity, mechanical properties which are similar to the apatite body in terms of chemical composition, but also it decreases the therapy course and bone repair significantly[30-32]. To date, various methods such as electrically [11, 32], freeze drying [33], solvent casting [22], fusion separation, and other methods for the construction of scaffolding for application in tissue engineering by researchers has been studied. In 2009, a study was conducted on the effect of fluoride additive on the mechanical properties of hydroxyapatite/alumina composites for increasing the strength of the scaffold [18, 20, 34]. Researchers have been studying the effects of MgF2 on animal skin and have not reported any toxicity [19]. Synthesized hydroxyapatite nanoparticles was done by adding of NaF and carbonate. Hydro-deformed apatite had increased the formation of the diameter of the apatite layer between the scaffold and the bone [13, 20]. In 2017, a study was conducted on the mechanical and cytotoxic properties of 3d printed multi-compartment capsular devices. The results confirmed that, the scaffold containing 15% of hydroxyapatite had more mechanical and biocompatible properties [35]. The researchers conducted a study on the construction of a hydroxyapatite-gelatin scaffold for bone reconstruction on rat rats. It was observed that, the use of this scaffold increased the speed of repair of bone tissue [35]. Moreover, the researchers constructed a composite scaffold of chitosan / polyvinyl alcohol / carbon nanotubes by electrostatic method. Polyvinyl alcohol was used as a surfactant to stabilize carbon nanotubes [36].
This study has driven us to verify and prepare nanocomposite of HA- Al2O3 with different additives and then, the chitosan/ HA- Al2O3 scaffold was systematized. The novelties of this research are investigating the effects of NaF and MgCl2.6H2O on preparing the nanocomposite of HA- Al2O3 as well as on the morphology and the microstructure properties of produced nanocomposite. Also, preparing the scaffold of chitosan / HA- Al2O3 as well as the microstructure, mechanical, cell viability and compatibilities of produced scaffold were investigated.
2-Experimentals
2.1-Preparation of Hydroxyapatite-Alumina nano composite powder:
Hydroxyapatite-alumina nano composite powder was prepared by precipitation method.
At first, suspension of 0.4 M Ca (NO3)2 4H2O (Merck, prolabo 0308821 142) and (NH4)2HPO4 (Merck, prolabo A0143307 037) was prepared. Then, 0.239 M (NH4)2 HPO4 solution was added drop wise to Ca (NO3)2 4H2O solution and stirred for 2 h and added to first solution (solution 1). Next, MgCl2.6H2O and NaF additives with weight percent of 10 wt% were added to solution 1[30]. In the next step, aluminum nitrate (LobaChemie 7784-27-2) was prepared in distilled water and mixed for 1 h (solution 2) and aged for 24 h. Then, the second solution was added to the first solution. The final solution was mixed for 2 h and aged for 24 h. After filtering and washing, the materials were dried and calcined at 1200 for 1 h.
2.2 Preparation of chitosan/ HA- Al2O3 scaffold
In order to build the scaffolding, the freeze casting method was used. At first, 2 gr chitosan was dissolved in100 ml of acetic acid solution of 1 % at 75 ° C for 30 minutes and then 0.4 gr gelatin was added and homogenized at 100 ° C for 12 h. Then, 25% of hydroxyapatite /alumina with two different additives powder made in the previous steps was added to the hydrogel and homogenized for 48 h at 120 ° C. After that, the sample was transferred to a 24-house dish and placed at an initial temperature of -20 °C for 24 h for initial freezing. Then, the scaffold was prepared in two freeze-dried steps. In the first stage, it was placed in the freezer dryer for 24 h at a temperature of -80 °C and placed in the glutamate solution of 25% for 24 h after leaving the scaffold. Then, after two washing steps with ethanol of 96% and hot water, the scaffold was again placed inside the freezer for 24 h. X-ray diffraction (XRD, PW1800, Philips) was used for phase identification.
A crystalline size of powders was determined by the Scherrer method as follow:
t = 0.89 λ / β cos θ (1)
Therefore, t is grain size, the wave length is λ and β is peak width and the angle in degrees is θ [30]. Field emission scanning electron microscope (FESEM) and transition electron microscopy (TEM, PHENOM) were conducted for investigation of microstructures and morphology of powders. Test samples were loaded at a testing machine (Instron 5569, Instron corp., Canton, U.S.) to measure the compressive strengths at a crosshead speed of 1 mm/min.
The apparent density and porosity of nano composite was measured using the Archimedes method. In the next step, the proliferation and survival of L929 cells on the surface of the samples were evaluated by MTT (3-(4,5-Dimethylthiazol-2-Yl)-2,5-Diphenyltetrazolium Bromide ) assay. To prepare the samples, a common protocol for this test was used. In this way, 5 mg of each of the samples was mixed in the medium and incubated at 37 ° C for 72 h. These samples were filtered to prevent contamination. After extracting the cells desired in the culture plate, number of wells was considered as controls and some were considered as the test samples. After the desired time, the culture medium was discarded and a certain volume of solution was spilled on the cells and then, the cells were incubated in this solution. At this time, the MTT ring was broken, breaking the ring created crystalline purplish color. The amount of this color was directly related to the living cells. Next, the supernatant was discarded and the cells were washed. At the end, the absorbance of the solution was calculated by the spectrophotometer.
The following formula is then used to determine the survival rate:
(2) Cell Viability% =
ODs Optical Density Sample, ODc Optical Density Control [2].
Cell culture and cell membrane propagation were used on scaffolds from the rats' tail (929L) cells. In the next step, the proliferation and survival of L929 cells on the surface of the samples were evaluated by MTT assay [5, 31]. Statistical comparison of data from t-student method was performed. All experiments were assayed in triplicate.
3-Results and discussions:
3.1. Synthesis of Hydroxyapatite Alumina nano composite powder with different additives:
The XRD pattern of the HA- Al2O3nano composite powders with and without additives was shown in Fig 1. The XRD pattern in Fig 1 indicated that, the samples was mostly HA and another crystalline phase of Tricalcium phosphate phase (T) existed (Sample H) . By adding of 10% MgCl2.6H2O, the Magnesium phosphate (M) was formed (Sample J) and with addition of 10% NaF, the formation of Sodium fluorophosphates (N) was achieved (Sample M).
Fig 1:X-ray diffraction pattern of the HA-Al2O3 nano composite powders with and without additives
The crystalline sizes and crystalline degrees of HA-Al2O3 nano composite powders with and without additives were explained at table 1.
Table 1: Comparing the crystalline sizes of H, J and M samples
Crystalline Degree (%) | Crystalline size (nm) | Sample |
71
76
84 | 54 nm
41nm
35 nm | Sample H
Sample J
Sample M |
As table 1 indicated, by increasing the MgCl2.6H2O, the crystalline sizes were reduced and crystalline degrees of nanocomposites increased which was due to the replacement of Cl- to OH- in HA crystal. By increasing MgCl2.6H2O, decomposition of HA decreased; therefore, the intensity peaks of HA phase increased. Also, by increasing NaF, the crystalline sizes decreased and the crystalline degrees of nanocomposites increased something which was due to the replacement of F- to OH- in HA crystal. By increasing NaF, decomposition of HA decreased and an intensity peak of HA phase was increased. Moreover, NaF as an additive had better effect on decreasing of crystalline size than MgCl2.6H2O, because the grain boundaries of NaF particles could prevented the growth of HA.
Fig. 2: FTIR curves of the HA- Al2O3 nano composite powders with and without additives
FTIR curves powder samples H, M and J were seen in Fig 2. The peak in the wave number of less than 500cm-1 was related to Al-O bond. The peak of P-O was related to phosphate groups at crystalline hydroxyapatite network in the wave numbers of 695 cm-1 and 831cm-1 the appeared peaks of J sample was related to the stretching vibration of Mg-O-Al bond. Peaks performed in 842cm-1 at FT-IR spectrum of H sample and peaks in the wave number of 831cm-1, 964 cm-1 at FT-IR spectrum of sample J were belonged to the Al-O bond stretching vibration [30]. At the wave numbers of 964cm-1 and 960cm-1 the peaks related to Al2O3 phase were appeared with the addition of 10% MgCl2.6H2O and NaF, respectively. Moreover, peak marked with P-H at the area of 2924cm-1 in the spectrum of sample of H and wave number of 1997cm-1 at FT-IR spectrum samples of J and wave number of 2005cm-1 at FT-IR spectrum samples of M were related to HPO4-2 groups [9].
3.2- Morphological properties of the HA-Al2O3 nano composite powder with different additives
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Fig 3: FESEM images of sample H, J and sample M after calcination at 1200 ℃ temperature for 1 h
Fig .3 shows the field emission scanning electron microscopy (FESEM) image of H, J and M samples with good dispersion and regular shape. Porous appearance with some agglomeration was seen in sample H. In sample J, in the presence additive of MgCl2.6H2O, particles with porous form indicated pirohydrolysis of magnesium chloride which resulted in the production of HCL gas that increased the pores and cracks in the surface of samples. However, in sample M had less porous appearance and with spherical shape.
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Fig 4: TEM images of sample H, J and sample M after calcination at 1200 ℃ temperature for 1 h
Transmission electron microscopy (TEM) images of samples H (HA-Al2O3 nano composite powder), J (HA-Al2O3 nano composite powder with 10% of additive MgCl2.6H2O) and M (HA-Al2O3 nano composite powder with 10% of additive NaF ) were used for investigating the particle size and morphology of nano composite powders in Fig 4.
As Fig 4 shows, the size of nanoparticles of sample H was about 50 nm with regular shape and some agglomeration. In sample J, in the presence additive of MgCl2.6H2O, particles formed with the sizes less than 45 nm and regular geometric shape; however, there was some agglomeration. In samples M, in the presence of surfactants and additive of NaF, the particle size was about 30 nm with regular geometric shape and without any agglomeration.
3.3 Morphological study of scaffold surface
The microstructures of the prepared scaffolds from the freewheeling casting method were studied by screens of field scanning electron microscopy (FESEM). As it was seen in FESEM images, the surface of all samples was completely porous. The existence of macroscopic cavities inside the scaffold created an interconnection between the porosity of the scaffolds. This interconnection was a vital parameter for cell infiltration, cell-to-scaffold attachment, nutrient transfer, and waste removal from metabolism and cell migration across a three-dimensional scaffold in the first days of placement of scaffold in the body. Another key parameter, in making the ideal scaffold was to apply porosity to texture engineering. The diameter of the porosity did not too large therefore, the cell could not attach to the wall of the scaffold for penetrating and growing. FESEM images in Fig 5 showed that, the size of porosity of SMA scaffolds (scaffold of chitosan / H A-Al2O3 with 10 % MgCl2.6H2O ) was in the range of 100-150 μm which was the required porosity for bone application. Investigating the FESEM images of SFA scaffold (scaffold of chitosan / HA-Al2O3with 10 % NaF) indicated the connection between the porosity of the scaffold and illustrated a significant increase in the internal connection of porosities (Fig 5.b).
Fig.5: FESEM images a) SMA b) SFA c) SHA scaffolds
Porosity measurement in this scaffold was indicated an increase in the diameter of the porosity of SFA scaffold compared to the SMA scaffold sample. The evaluation of SHA scaffold (scaffold of chitosan/ HA without additives) has shown that the various difference compared to other samples, especially in SFA scaffold. This difference was due to, the stronger binding of fluorine to the amine chitosan group relative to the hydroxide linkage with the amine group. In general, previous studies have shown that, the addition of nanoparticles into scaffolds led to a reduction in the porosity size which related to the study on chitosan gelatin scaffolds containing tricalcium phosphate nanoparticles and identified the addition of nanoparticles caused to reduce the porosity from about 128 to 157 µm to 104 to 137 µm [4, 26 ].
3.4: Porosity percentage of scaffolds
Another important parameter on the scaffold properties is the porosity of the scaffold, which has a great impact on mechanical properties and being biocompatible. In order to calculate the porosity of scaffolds, the Archimedean method is used [31].
Studies have shown that, the porosity requirement for bone tissue for the correct reconstruction of normal bone tissue was about 45% to 65%. Low porosity prevented food from feeding, migrating, and disposing of appropriate cell materials. Also, the porosity percentage of extremely high scaffolding reduced the mechanical properties of the scaffold. Previous studies have shown that, the addition of ceramic particles could reduce the porosity and increase the strength of scaffold. Table 2 shows the porosities of the SHA, SFA, and SMA scaffolds. As it was shown, the porosity percentages of all scaffolds were within the porosity percentage required for bone scaffolds. However, the SMA scaffold with 70% porosity had the highest porosity percentage. Although this porosity could have the best effect on the survival rate of the cell and reduce the mechanical properties of the scaffold. Also, the SFA scaffold had 63% porosity, which was due to a stronger connection to the fluorine bond that confirmed the results of the presence and linkage of NAF and MgCl2.
Table 2 : The porosity percentages of different scaffolds
Porosity percentages (%) | Sample |
3%70 |
SMA
|
4%63 | SFA
|
3%56 | SHA |