Cytotoxicity evaluation of self-etching dentine bonding agents in a cell culture perfusion condition.

OBJECTIVE: The aim of this study was to evaluate the cytotoxicity of three dentine bonding agents (G-Bond, Clearfil S(3) Bond and Clearfil SE Bond X) in cell-culture perfusion.
METHODS: In this experiment, 8×10(4) TCPC SV40 cells (bovine-pulp-derived cells transfected with simian virus 40 large T-antigen) in MEM-alpha media, 20%FCS were seeded on mesh in a 6-well plate and incubated at 37 °C with 5% CO(2). After 2 days, the mesh inserts were transferred to a 24-well plate and incubated in MEM-alpha media, 20%FCS with 50 μg/ml of ascorbic acid at 37 °C with 5% CO(2) for 14 days. The test materials were applied to the dentine discs of dentine barrier models. Three-dimensional cell cultures in mesh and perfusion conditions were generated in this experiment. Each material, as well as the negative control (President) and the positive control (vitrebond), was tested in 5 models with the tests repeated in triplicate. The MTT assay was used to determine cell viability after the diffusion of leachable toxicity from the tested materials through the dentine discs.
RESULTS: The cell survival rate with G-Bond and Clearfil S(3) Bond was 113.03 and 90.98 percent, respectively, whereas that with Clearfil SE Bond X was 111.83 percent. All three dentine bonding agents had no toxicity compared with the negative control group (P>.05).
CONCLUSIONS: All three self-etching dentine-bonding agents are nontoxic. Pulp damage caused by these three bonding agents is unlikely to occur in the clinic.

INTRODUCTION

Dentine bonding agents are bonding agents that consist of 3 parts: (i) an acid that removes the smear layer accumulated on the dentine and that helps increase the microporosity of the enamel (etching step), (ii) a substance that enhances the flow of bonding agents into the dentine and increasing the microporosity of the enamel by modifying dentine as a bonding substrate (priming step), and (iii) the bonding agents (bonding step). Traditionally, the use of dentine bonding agents required the use of all three of these steps. Recently, however, dentine bonding agents have been developed that reduce the process to only one or two steps, resulting in faster and more convenient application. Selection of a dentine bonding agent requires the consideration of the bonding properties (i.e., how effectively the bonding agent can bond the dental restorative material to the dentine) and the cytotoxicity of the dentine bonding agents.1–2

In a previous study, the cytotoxicity of three dentine bonding agents was determined using the agar overlay technique.3 The results showed that the toxicity of G-Bond and Clearfil S3 Bond diffusing into the agar medium was moderate whereas that of Clearfil SE Bond X was high. The study also found that the three dentine bonding agents yielded the same lysis index (i.e., 1). This result revealed that the three dentine bonding agents have low toxicity according to the ISO/FDIS 7405:2008 (E) Standard, which is based on an in vitro evaluation of the biocompatibility of medical devices used in dentistry.4 However, the agar overlay technique only allowed a preliminary cytotoxicity evaluation and did not reveal the percentage of surviving cells. The results only indicated the cytotoxicity of the tested dentine bonding agents.

It is advisable to evaluate the biological properties of dentine bonding agents that are in close contact with dentine prior to using them in patients. According to the ISO 7405:1997 Standard, an in vitro evaluation of the biological properties of dentine bonding agents (e.g., cytotoxicity evaluation through a cell-culture test) is the primary method used to evaluate the cytotoxicity of such agents.5 Originally, researchers used cell-culture tests to evaluate the biological properties of dental materials.6 The agar overlay method and the Millipore filter method were introduced to simulate the material-cell contact interaction.7–8 However, the agar and filter methods still did not simulate dentine in vivo clinically. In 1977, the model cavity system was introduced to better simulate the clinical situation.9 The test material was separated from the cells by either a synthetic filter or a dentine slice. Most subsequent in vitro models were based on the use of human dentine. An in vitro test system using dentine for the evaluation of toxicity has been reported.10–12 In these studies, the toxic products of materials that diffused through the dentine were diluted in at least 2.5 ml of cell culture medium before contacting the target cells. However, in a clinical situation, the leachable toxic product will have a direct effect on the cells of the pulp, which lie close to the dentine.

In 1996, a dentine barrier model for the cytotoxicity evaluation of dental cement was reported.13 This model is based on a commercially available device and is considered to be an important prerequisite for a standard test. In this model, the cells were seeded on the pulp side of the dentine and were placed above the cell culture medium. This in vitro pulp chamber simulated in vivo conditions. Our study used a dentine model and three-dimensional cell cultures that have been previously described by Ulker and Sengun.14

Cell perfusion was limited by the blood circulation inside the tooth cavity and was equal to 20-82.4 ml/min/100 grams of tissue.15 It has been reported that perfusing the chamber with 5 ml medium/h did not decrease toxicity but can lead to increased cell death or cell disruption.16 Therefore, in the present study, the perfusion conditions included a cell feed flow rate of 2.0 mL/h. At this flow rate, cells have a higher survival rate than those cultured under static conditions. This difference may be because this rate mimics the blood flow within the pulp chamber, where cytotoxic leaching occurs.

The aim of this study was to evaluate the cytotoxicity of three self-etching dentine-bonding agents (G Bond, Clearfil S3 Bond and Clearfil SE Bond X) with a three-dimensional cell culture and perfusion conditions that were not used in the previous study.3 The hypothesis tested was that different self-etching dentine bonding agents have different cytotoxic profiles.

MATERIALS AND METHODS

Test materials

Three self-etching dentine bonding agents were used in this study. G Bond, Clearfil S3 Bond and Clearfil SE Bond X were the experimental materials. The negative and positive controls were President (Coltene AG, Alstatten, Switzerland) and Vitrebond (3M Medica GmbH, Germany), respectively. Material compositions, manufacturers and batch numbers are shown in Table 1.

Table 1.

Material composition, manufacturers and batch numbers.

Material	Manufacturer	Composition	Batch #
G-Bond™	GC Corp, Tokyo, Japan	4 –MET monomer, Phosphoric acid, Acetone, Water, UDMA, Silica	603291
Clearfil™ S3 Bond™	Kuraray Medical Inc, Okayama, Japan	MDP, Bis-GMA, HEMA, Hydrophobic dimethacrylate, Di-camphorquinone, Ethyl alcohol, Water, Silanated colloidal silica, Hydrophilic monomer	00045 A
Clearfil™ SE Bond™ X	Kuraray Medical Inc, Okayama, Japan	Primer: MDP, HEMA, Di-camphorquinone, Water Bonding: Bis-GMA, MDP, HEMA, Di-camphorquinone, Silanated colloidal silica	00603 A (Primer)00852 A (Bonding)
President (Negative Control)	Silicone impression material	Coltene AG, Alstatten, Switzerland	MJ938
Vitrebond (Positive Control)	Light-curing glass Ionomer cement	3M Medica GmbH, Broken, Germany	20040517

Mesh preparation

Polyamide (diameter 8 mm) was etched with 0.1 M acetic acid for 30 min, washed with sterile water 3 times and sterilized by autoclaving (Hirayama, Tokyo, Japan) before the experiment. The mesh was coated in fibronectin (0.03 mg/ml in water), and the mesh was left to dry for 2 h in a bio-hazard safety cabinet.

Cell preparation

The target cells used in this experiment were TCPC SV40 (bovine fibroblast pulp-derived cells transfected with simian virus 40 large T-antigen).16 A 1.25-ml volume of MEM-alpha (Minimum Essential Media, Gibco, New York, USA), including 20% fetal calf serum, was added to each well of a 6-well tissue culture plate. Then, a Millicell membrane (Minucells and Minutissue, Bad Abbach, Germany; size 30 mm, pore size 0.45 μm) was inserted in each well.

Four dried meshes were placed in each insert. A 20-μl aliquot containing 4×106 cells/mL was dropped on each mesh in the insert. The plate was incubated at 37o C with 5% CO2 and 100% humidity for 48 h. Then, each mesh was separately placed into the wells of a 24-well tissue culture plate. The cells on the meshes were fed with 1 ml of MEM-alpha media, 20%FCS containing 50 μg/ml of ascorbic acid, and the medium was changed every other day. After growing for 14 days in the incubator, the three-dimensional cell cultures on the meshes were ready for use in the experiment (Figure 1).

Figure 1.

Cell culture on mesh after incubation for 2 days, 7 days, 10 days and 14 days, observed using an inverted microscope. (Mag. 10×).

Dentine disc preparation

A dentine disc that was 500 ± 25 μm thick and that was close to the pulp cavity was longitudinally sectioned from a bovine incisor. A dentine disc with a diameter of 6–7 mm under the cementoenamel junction was cut for the experiment. The pulp side of each disc was etched with 50% citric acid for 30 s, soaked in normal saline and autoclaved before the experiment (Figure 2).

Figure 2.

Schematic illustration of the bovine tooth dentine slices (a) Longitudinal section of 500±25 μm thickness (b) 5 × 5 mm2 section at the level of the cemento-enamel junction

In vitro perfusion chamber

A commercial cell culture chamber (Minucells and Minutissue, Bad Abbach, Germany) was used for the in vitro model.16 The chamber was separated into a pulp side and a cavity side by the dentine disc mentioned above. The pulp side of the disc was placed over the cultivated cell mesh, and a stainless steel clamp held the 2 compartments together. Cells in the mesh were fed with MEM-alpha media, 20%FCS that was contained in the lower part of the chamber. The model was placed on a hot plate (37 ± 2 °C), and culture medium was perfused through the lower part of the chamber. Each dentine bonding agent as well as the negative and positive control was tested in 5 cell culture chambers. All experiments were repeated in triplicate. The perfusion pump (Ismatec UK Co. Weston-super-Mare, England) was connected and adjusted to a perfusion rate of 0.2 ml/h for 24 h before application of the test material (Figure 3). A cotton pellet soaked with culture medium was placed on the dentine of the cavity side.

Figure 3.

Perfusion conditions.

The test procedure

After 24 h of perfusion, the perfusion rate of the medium was adjusted to 2 ml/h to simulate blood flow in the pulp. The cotton pellet in the cavity side was removed. The dentine in the cavity side was cleaned with sterile water and dried with gently blown air. Three self-etching bonding agents as well as the President and Vitrebond controls were applied to the dentine according to the manufacturers’ recommendations. The enzymatic activity of target cells was analyzed using the MTT (3-(4,5-dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide) assay after 24 h of test material exposure.

MTT assay

The mesh was removed from the stainless-steel holder of the perfusion chamber and immediately inserted into 0.5 ml of freshly prepared MTT solution (1 well/1 mesh) in a 48-well tissue culture plate. The plates were incubated for 2 h. Mitochondrial dehydrogenase in living cells converts the yellow water-soluble tetrazolium salt 3-(4, 5-dimethylthiazol-2-yl)-2, 5 –diphenyltetrazolium bromide into dark blue formazan crystals that are stored in the cytoplasm of the cells. Then, the MTT solution was removed, and the mesh was washed twice with 0.5 ml of phosphate-buffered saline solution. Dimethyl sulfoxide (DMSO; 250 μl) was added to each well to dissolve the formazan. The plate was agitated on a shaker for 30 minutes to enhance the dissolution of the formazan. A 200-μl aliquot was drawn from each well and transferred to a 96-well tissue culture plate. The spectrophotometric absorbance was measured at 540 nm, using DMSO as the blank.

Statistical analysis

The mean optical density of the negative control group was set to represent 100% viability. The results for the experimental groups and the positive control were expressed as the percentages of the negative control. The statistical analysis was performed by applying the non-parametric Mann-Whitney test (P<.05).

RESULTS

The percentages of viable cells compared to the controls for G Bond, Clearfil SE Bond X and Clearfil S3 Bond are shown in Figure 4. The average percent cell viability after exposure to G Bond, Clearfil SE Bond X, Clearfil S3 Bond and Vitrebond was 113.03, 111.83, 90.98 and 59.90, respectively. Vitrebond was more toxic than G Bond, Clearfil SE Bond X and Clearfil S3 Bond (P<.01), whereas the experimental group did not have any toxicity compared with the negative control group (P>.05).

Figure 4.

Cell viability percentages after testing with self-etching dentine bonding agents, positive controls and negative controls. (different superscript letters signify P<.05)

DISCUSSION

In a previous study, the cytotoxicity levels of self-etching dentine-bonding agents (G Bond, Clearfil SE Bond X and Clearfil S3 Bond) were evaluated using the agar overlay technique. This analysis showed that the G Bond and Clearfil S3 Bond were both moderately cytotoxic, whereas the Clearfil SE Bond X appeared to be more toxic than the other 2 bonding agents. The amount of cells destroyed by each of the three dentine bonding agents was not significantly different.3 Because this was only a preliminary evaluation of the cytotoxicity of the three dentine-bonding agents, it was not possible to determine the level of toxicity quantitatively. Hence, a qualitative study of a dentine barrier model simulating clinical practice was needed to obtain reliable data. This study revealed that the percent of viable cells for G Bond, Clearfil S3 Bond and Clearfil SE Bond X was 113.03, 90.98 and 111.83, respectively.

In this study, three dentine bonding agents were studied under two systems. G-Bond and Clearfil S3 Bond were processed in one step, and a two-step system was used for the self-etching primer bonding system of Clearfil SE Bond X. In the all-in-one system, the etching, priming and bonding steps are combined together as one step for resin-bonding. In contrast, in the two-step self-etching primer bonding system, the etching and primer steps are combined together as a single step that is separate from applying the resin bonding agent prior to restoration of the tooth with a resin composite. In the Clearfil S3 Bond experiment, cell viability was 90.98%. This value was lower than the other groups, but the difference was not statistically significant. The difference may be due to the presence of hydrophobic dimethacrylate in the composition. Hydrophilic monomers such as HEMA or TEGDMA have been shown to be cytotoxic, but to a lesser degree than a more hydrophobic monomer.17 However, self-etching adhesive systems were less cytotoxic than the total-etching system.18

The preparation of materials for experiments significantly has been reported to alter the apparent cytotoxicity of the materials.19 Thus, every effort was made to simulate in vivo conditions in the laboratory. However, it is not possible to create an environment that totally replicates clinical conditions. Cell toxicity assays have been performed both in cell lines and primary cells, but immortalized cell lines are more stable than primary cells.20

No differences have been observed in the growth of bovine pulp-derived cell lines transfected with simian virus that were seeded on dentine discs and those seeded on tissue culture plates.21 Scanning electron microscopy (SEM) also showed biocompatibility between the dentine and cells. Thus, bovine teeth are an appropriate choice for use with the bovine pulp cell line in this experiment.

It has been demonstrated that 0.5 mm of dentine can reduce material toxicity to 75% and that 1 mm of dentine can reduce toxicity by up to 90% of the control value (i.e., the value obtained when dentine was not present).22 Most cytotoxicity research uses 500 μm for the standard thickness of the dentine barrier slice in the pulp chamber model.23 The permeability of the dentine varies in different regions of the tooth. Therefore, the region of dentine that is selected is important when evaluating restorative materials in terms of bond strength and cytotoxicity. Maroli et al24 showed, using scanning electron micrographs, that there are more tubular openings in the cervical third of approximal sections than in occlusal and middle. The cervical area of the bovine tooth was used as the dentine barrier in this experiment. With respect to transdentine permeability characteristics, bovine dentine at the level of the cemento-enamel junction seems to be a suitable alternative for coronal human dentine.25

The use of perfused dentine barrier models is a widely accepted method of evaluating the biological properties and the toxicity of dental restorative materials that will come into contact with dentine. However, each step of these experiments must be performed cautiously. If contamination occurs during the experiment, the experiment will be ineffective because the complete growth of the cell culture in the mesh requires 14 days. Moreover, researchers must have adequate experience with and knowledge of 3-D cell culture techniques. Each step requires meticulous technique, especially the installation of the perfusion system, which is a 3-way connection with a flow rate similar to blood flow in the actual pulp. The results from such experiments are similar to clinical conditions and are reliable. Another advantage of this study was the ability to reduce the quantity and frequency of animals used in experiments. An experiment with animals is needed when the results from of in vitro studies are ambiguous. In accordance with the first priority of ISO 7405, it is recommended to avoid the use of animals for experiments if the study can possibly be conducted in vitro.

CONCLUSION

All three self-etching dentine-bonding agents were non-toxic compared with the negative control group (P>.05). These agents could be used clinically in cases where there is more than .5 mm of remaining dentine above the pulp.