Poly(N-isopropylacrylamide-co-N-tert-butylacrylamide)- grafted hyaluronan as an injectable and self-assembling scaffold for cartilage tissue engineering

Abstract

Novel poly(N-isopropylacrylamide-co-N-tert-butylacrylamide)-grafted hyaluronan [P(NIPAAm-co-NtBAAm)-g-HA] has been developed as a modified derivative to improve phase-transition characteristics of PNIPAAm-g-HA, which has a lower critical solution temperature (LCST) of approximately 32°C. This promising self-assembling biomaterial has potential as an injectable scaffold for in situ cartilage tissue engineering. LCST of the P(NIPAAm-co-NtBAAm)-g-HA decreased to approximately 3.6°C compared to that of the original PNIPAAm-g-HA. This modification enabled self-assembly at body temperatures lower than the temperature of the parental PNIPAAm-g-HA molecule. Cytotoxicity and acute systemic toxicity assays revealed that P(NIPAAm-co-NtBAAm)-g-HA was not hazardous. The DNA content of chondrogenic differentiated mesenchymal stem/stromal cells (MSCs) embedded in the gels was higher than that of biomaterial-free aggregates during the culture periods. Cartilage-related genes were also expressed in chondrogenic differentiated MSCs embedded in the P (NIPAAm-co-NtBAAm)-g-HA hydrogel. Specifically, an increased expression of SRY-related HMG box-containing gene 9 (Sox9) observed in the hydrogel group compared to controls. These data suggest that P(NIPAAm-co-NtBAAm)-g-HA is a promising injectable scaffold with thermoresponsive properties suitable for in situ cartilage tissue engineering.

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Muramatsu, K. , Saito, Y. , Wada, T. , Hirai, H. and Miyawaki, F. (2012) Poly(N-isopropylacrylamide-co-N-tert-butylacrylamide)- grafted hyaluronan as an injectable and self-assembling scaffold for cartilage tissue engineering. Journal of Biomedical Science and Engineering, 5, 639-646. doi: 10.4236/jbise.2012.511079.

1. INTRODUCTION

Cartilage tissue engineering using autologous chondrocytes (or mesenchymal stem/stromal cells (MSCs) as a cell source) has been developed, and has been used in clinical applications. In the original system of chondrocytes implantation, a cell suspension of autologous chondrocytes expanded in monolayer culture was transplanted into defective articular cartilage under a cover of periosteal flap [1-3]. This was a pioneering system, with great promise for cartilage repair, although it had some disadvantages. These disadvantages included leakage of cells from the transplanted site and uneven distribution of the transplanted cells in the site due to gravity [4]. In the improved second generation of chondrocyte implanttation systems, tissue-engineered cartilage was prepared using in vitro three-dimensional culture of atelocollagen gel scaffolds embedded with chondrocytes or mesenchymal cells [5-7]. A number of other biodegradable scaffolds have also been studied for cartilage tissue engineering. Most of these scaffolds are gel or sponge forms made of collagen, gelatin, hyaluronan, chondroitin sulfate, chitin/chitosan, alginate, poly(lactide-co-glycolide), polycaprolactone, and their derivatives or composites [8-13]; these systems still require either a periosteal flap or substitute for fascia to cover engineered cartilage.

Current studies focus on the use of novel biomaterials possessing injectable and in situ gelling characteristics; these properties will facilitate minimally invasive procedures under microscopic surgery for chondrocyte transplantation. Thermoresponsive polymer-grafted polysaccharides, which have both the characteristics of biological activity derived from polysaccharides and the selfassembling ability of thermoresponsive units such as poly(N-isopropyl-acrylamide) (PNIPAAm), are biomaterials that could fulfill this purpose [14-16]. In particular, PNIPAAm-grafed hyaluronan (PNIPAAm-g-HA) has the ability to induce ectopic chondrogenesis in cooperation with transplanted chondrocytes and growth factors in animal experiments [16]. The strategy of graft polymerization and coupling of PNIPAAm to biomaterials is being rapidly adopted in biomedical field. For example, the self-assembling property of functional biomaterials can be exploited to develop drug delivery carriers and injectable scaffolds for tissue engineering, as well as for cell sheet engineering [14-19], because the lower critical solution temperature (LCST) of PNIPAAm in aqueous solution (approximately 32˚C) is suitable for self-assembly in physiological conditions. However, in cases where the local body temperature at the target site is close to the LCST of PNIPAAm, in situ gelation of injected PNIPAAm-grafted materials may be compromised in the target tissue. Thus, tuning of the LCST is critical for optimal thermoresponsive biomaterial function in tissue engineering applications. Reduction of polymer LCST is facilitated by copolymerization with more hydrophobic monomers, such as N-tert-butylacrylamide (NtBAAm) [20,21]. Indeed, the theoretical LCST of a homopolymer composed of NtBAAm is approximately –5˚C.

In the present study, we modified an injectable scaffold (PNIPAAm-g-HA) that we had previously developed for in situ cartilage engineering [16]. This was achieved by adding 5 mol% of NtBAAm to generate poly (NIPAAm-co-NtBAAm)-grafted hyaluronan [P(NIPAAmco-NtBAAm)-g-HA] (Figure 1). Biocompatibility of this novel biomaterial was evaluated in terms of cytotoxicity (colony-forming assay) and acute systemic toxicity assessment. To investigate its potential as a scaffold for cartilage tissue engineering, cartilage-related gene expression in chondrocytes embedded in the gel was also studied in vitro.

2. MATERIALS AND METHODS

2.1. Chemicals

N-isopropylacrylamide (NIPAAm), N-tert-butylacrylamide (NtBAAm), 2-aminoethanethiol hydrochloride (AET-HCl), and 2,2’-azobis(isobutyronitrile) (AIBN) were purchased from Tokyo Kasei Kogyo Co., Ltd. (Tokyo, Japan). 1-Ethyl-3-(3-dimethylamino-propyl)-carbodiimide hydrochloride (EDAC) was purchased from DOJINDO Laboratories (Kumamoto, Japan). Hyaluronic acid sodium salt from rooster comb, and other high-purity-grade reagents for chemical synthesis were purchased from Wako Pure Chemical Industries Ltd. (Osaka, Japan).

2.2. Preparation of Poly(N-Isopropylacrylamideco-N-tert-Butylacrylamide)-Grafted Hyaluronan [P(NIPAAm-co-NtBAAm)-g-HA]

Amino-terminated poly(NIPAAm-co-NtBAAm) [P(NIPAAm-co-NtBAAm)-NH2] was prepared by radical polymerization using AIBN as an initiator, as previously reported [16]. Briefly, NIPAAm/NtBAAm (5 mol% NtBAAm), AIBN and AET were dissolved in degassed DMF under argon-atmosphere, and the polymerization was conducted for 7 h at 70˚C. The product solution was dialyzed against ultrapure water by using spectra/Por 7 (MWCO: 8000) for 48 h and then lyophilized. Graftpolymerizations of P(NIPAAm-co-NtBAAm)-NH2 to hyaluronan (HA) were carried out using water-soluble carbodiimide agent in phosphate buffer. Hyaluronic acid sodium salt (100 mg) and P(NIPAAm-co-NtBAAm)- NH2 (500 mg) were dissolved in 0.05 M phosphate buffer (pH 6.0), and then, EDAC was added to the solution. The reaction was conducted at 24˚C with stirring for 48 h. To remove non-reacted P(NIPAAm-co-NtBAAm)- NH2, the reaction mixture was dialyzed against excess ultrapure water using spectra/Por 7 (MWCO: 25,000) for 48 h, lyophilized, and washed with acetone. The products were dried and stored at room temperature in a desiccator.

2.3. Low Critical Solution Temperature Measurements

The optical transmittance of polymers in deionized water was measured at 500 nm at temperatures ranging from 25˚C to 45˚C with a V-630BIO spectrophotometer (JASCO) to estimate the phase-transition temperature of the specimens. The low critical solution temperature (LCST) of the polymer solution was determined as previously reported [15,16].

Figure 1. Chemical structure of poly(N-isopropylacrylamide-co-N-tert-butylacrylamide)-grafted hyaluronan [P(NIPAAm-co-NtBAAm)-g-HA]. R = CH(CH3)2 or C(CH3)3 (NIPAAm/NtBAAm molar ratio of 95/5).

2.4. Cytotoxicity Test (Colony-Forming Assay)

Cytotoxicity of the P(NIPAAm-co-NtBAAm)-g-HA was evaluated by means of the colony-forming assay using the Chinese hamster lung fibroblast cell line V79 (obtained from Health Science Research Resources Bank, Osaka, Japan). V79 cells suspended in Eagle’s minimum essential medium (MEM) containing 5% fetal bovine serum (FBS) were seeded into 12-well culture plates (50 cells/well) and incubated for 24 h in an atmosphere of 5% CO2 in air at 37˚C. After 24-h incubation, the medium of each well was changed individually to the sample-solubilized medium (at 0, 0.1, 0.5, 1.0, and 5 mg/mL final concentration). The cells were cultured for a week, then fixed with methanol, and stained with 2% Giemsa solution (Wako, Japan). Subsequently, the number of colonies consisting of 50 cells or more was counted with Model CL560 colony counter (Sibata Scientific technology Ltd., Saitama, Japan).

2.5. Acute Systemic Toxicity Assessment

All animal experiments in this study were approved by the Animal Care Committee at Tokyo Denki University. Jcl/ICR mice (age 4 weeks) were purchased from Clea Japan, Inc. (Tokyo, Japan), and kept under a condition with standard light-dark schedule, relative temperature, and humidity for 7 days to adapt to their environment. P(NIPAAm-co-NtBAAm)-g-HA was administered with saline at a dose of 2 mg/g body weight by intraperitoneal injection into mice (n = 5). Each mouse was clinically examined, and body weight was measured once a day for the initial 3 days and every other day for the following 4 days. After the mice were sacrificed and inspected for visible toxic damage, extracted organs, including the heart, lung(s), liver, spleen, and kidney(s), were weighed using an electronic balance AUX320 (Shimazu Co., Kyoto, Japan). Tissues were fixed with 10% formalin neutral buffer solution, dehydrated in ethanol and xylene, embedded in paraffin, and sliced onto aminosilanecoated glass. The specimens were stained by hematoxylin-eosin, and evaluated by microscopic examination using a DX51 microscope equipped with a DP71 digital camera system (Olympus, Tokyo, Japan).

2.6. Isolation and Three-Dimensional Cultures of Bone Marrow Derived Mesenchymal Cells

Rabbit bone marrow-derived mesenchymal stem/stromal cells (MSCs) were harvested from femur and tibia of New Zealand White male rabbits (age 6 - 8 weeks). Briefly, after anesthesia by intravenous injection of Somnopentyl (Kyoritsu Seiyaku Co., Tokyo, Japan), bone marrow fluid in each incised long bone was aspirated or flushed out using an 18-gauge needle and syringe (Terumo, Tokyo, Japan) containing 20 units of heparin. The aspirate was suspended in serum-free DMEM/F12 medium (Invitrogen) and passed through a 100-μm-mesh cell strainer, collected by centrifugation, and resuspended in fresh DMEM/F12 medium containing 10% FBS. After cells were cultivated in a monolayer, cells at passage 2 were used for in vitro three-dimensional culture. A mixture composed of 50 μL of 1.5 wt% P(NIPAAm-co-NtBAAm)- g-HA and 5 × 105 MSC cells were mixed in centrifuge microtubes to embed the cells into hydrogels, and then, warmed culture medium was added to the tube. Cells embedded in P(NIPAAm-co-NtBAAm)-g-HA hydrogels were cultivated in DMEM/F12 supplemented with 10% FBS, 10−7 M dexamethasone, 10 ng/mL of transforming growth factor (TGF-β1), and ITS (10 μg/mL insulin, 6.7 mg/mL transferring, and 5.5 μg/mL selenium) for 4 weeks at 37˚C with 5% CO2. As a standard for chondrogenic differentiation, a gel-free cell aggregate (5 × 105 cells) was also prepared by centrifugation as a positive control.

2.7. DNA Assay

At each time point of cultivation, cells were rinsed with PBS and homogenized in 10 mM Tri-HCl (pH 8.0) containing 1 mM EDTA and 1% Triton X-100 to analyze DNA contents. Double-stranded DNA was measured using bisbenzimide dye (Hoechst 33258) (Bio-Rad, Hercules, USA) according to the manufacturer’s instructions.

2.8. Reverse Transcription-Polymerase Chain Reaction (RT-PCR)

Total RNA was extracted from cells by using ISOGEN RNA isolation kit (Nippon Gene, Tokyo, Japan) with DNase I treatment according to the manufacturer’s instructions. One microgram of each RNA sample was reverse-transcribed into cDNA by using SuperScript II first-strand synthesis system for RT-PCR (Invitrogen). To analyze expression of specific genes, equal amounts of first strand cDNA were amplified by PCR using Ex Taq polymerase (Takara Bio Inc., Ohtsu, Japan) and specific forward and reverse primers for each gene (Table 1). The PCR conditions were as follows: 1 min at 94˚C, 30 sec at 55˚C, and 30 sec at 72˚C for 32 cycles. The products amplified by PCR were subjected to electrophoresis in a 2% agarose gel, and digital photographs of ethidium bromide-stained gels were taken with an ImageQuant LAS4000 image analyzer (GE Healthcare).

2.9. Statistical Analysis

Student’s unpaired t-test or the Aspin-Welch paired t-test was employed for equal variance or unequal variance,

Table 1. Specific primers used in RT-PCR analysis.

respectively. Significant differences were determined at p < 0.05 for the t-test.

3. RESULTS

3.1. LCST of Synthesized P(NIPAAm-co-NtBAAm)-g-HA

The transmittance-temperature curve of the 0.5 wt% of thermoresponsive polymer-grafted HAs in aqueous solution is shown in Figure 2. The LCSTs of PNIPAAm-gHA and P(NIPAAm-co-NtBAAm)-g-HA were 32.0˚C and 28.6˚C, respectively (Table 2). These LCSTs were almost same as the LCST of each N-substituted acrylamide polymer itself.

3.2. Cytotoxicity Evaluation

The cytotoxicity of thermoresponsive-polymer-grafted HA derivatives was evaluated using a colony-forming assay. Colony-forming efficiency (CFE) of the HA derivatives is shown in Table 2. No cytotoxicity was detected over a range of concentrations up to 1 mg/mL, whereas a slight reduction in CEF was observed in all samples at the recommended maximum concentration (5 mg/mL). However, the values of 2 thermoresponsive polymer-grafted HA derivatives were higher than the value of unmodified hyaluronan.

3.3. Acute Systemic Toxicity Analysis

There were no obvious clinical signs related to the effects of intraperitoneal injection of P(NIPAAm-coNtBAAm)-g-HA in mice. Body-weight gain during the study did not differ between the control and sample injection group (Figure 3). The Summary of relative organ weights and histopathological findings of test animals are shown in Table 3; no significant differences were de-

Table 2. Characteristics of thermoresponsive polymer-grafted hyaluronan derivatives.

Figure 2. Transmittance as a function of temperature for (●) P(NIPAAm-co-NtBAAm)-g-HA with NIPAAm/NtBAAm molar ratio of 95/5, (■) PNIPAAm-g-HA, and (▲) hyaluronan (HA).

Figure 3. Body weight change of mice administrated P(NIPAAm-co-NtBAAm)-g-HA by intraperitoneal injection with saline at dosage of 2 mg/g body weight for a week. ●: P(NIPAAm-co-NtBAAm)-g-HA, △: control.

Table 3. Summary of relative organ weights and histopathological findings of mice injected with P(NIPAAm-co-NtBAAm)-g-HA.

tected between the groups. Figure 4 shows typical histological photographs of liver of mice 7 days after injection of P(NIPAAm-co-NtBAAm)-g-HA. We did not detected signs of inflammation or any other remarkable differences in comparison with normal tissue (control groups).

3.4. DNA Assay

Figure 5 shows the DNA content of MSCs in chondrogenesis at each time point. A transient increase in DNA content (indicative of proliferation) in response to TGF-β was observed in the P(NIPAAm-co-NtBAAm)-g-HA gel group at day 7, whereas no cell expansion was observed in gel-free aggregates at the same time point. Although DNA content at day 14 decreased relative to day 7 in both experimental groups, the initial amount was maintained for at least 14 days in the gel group only.

Conflicts of Interest

The authors declare no conflicts of interest.

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