2.1

Reagents

Bis-GMA (2,2-bis[4-(2-hydroxy-3-methacryloyloxy propoxy) phenyl] propane), HEMA (2-hydroxyethyl methacrylate), 2-MP (bis[2-(methacryloyloxy) ethyl] phosphate, TCDM di(hydroxyethyl methacrylate) ester of 5-(2,5,-dioxo tetrahydrofurfuryl)-3-methyl-3-cyclohexenyl-1,2-dicarboxylic acid), and TEGDMA (triethylene glycol dimethacrylate) were purchased from Sigma Chemical (St. Louis, MO, USA) and used without further purification ( Table 1 ).

Low-electroendosmosis agarose gel D-1 (EEO = 0.09–0.13 by Weime method; sulfate < 0.14%) with a gelling temperature of 36–39 °C, a melting temperature of 87–89 °C, and a gel strength of 1.200 g/cm ² was purchased from Shelton Scientific Inc (Shelton, CT, USA).

2.2

Experimental procedures

Agarose gel powder (0.5 g) was suspended in 100 mL of aqueous buffer at pH 3.1 (2.1% citric acid/1% sodium citrate), 6.3 (1% citric acid/2.9% sodium citrate), 8.5 (3.8% sodium tetraborate boric acid), or 12.3 (0.4% sodium hydroxide). Each buffer was precisely titrated to its nominal pH with HCl 4 N before use. Each agarose gel suspension was heated at full power in a 500-W microwave oven for 2 min to completely solubilize the agarose, poured into a horizontal 10-well electrophoretic cell (Owl EasyCast Horizontal System B1, Thermo Scientific, Portsmouth, NH, USA), and allowed to cool to room temperature. The final gel dimensions were 9 cm × 11 cm, and electrophoresis system buffer capacity was 600 mL. The tested monomers (bis-GMA, HEMA, 2-MP, TCDM, and TEGDMA) were dissolved in ethanol at 5% (w/w) concentration.

A voltage of 50 or 100 V was applied to the cell electrodes using a DC Power Supply (Apelex PS304 MinipacII, Massy, France), and both current and voltage were monitored during experiment. NaCl was added to the buffer used for electrophoresis to adjust their ionic strength to maintain the same electrical current/intensity ratio for all tests without monomer addition (data not shown). The buffers were adjusted so that the current at 100 V was 100 mA (highest ionic strength), 50 mA, or 25 mA (lowest ionic strength).

The dissolved monomers (10-μL aliquots) were injected into the wells of the gel, and voltage was applied for 30 min. After electric field application, the gel was carefully removed from the electrophoretic cell and placed onto a layer of polyethylene film on top of a silica thin-layer chromatography plate (Sigma Chemical) ( Fig. 1 ). The silica plate was used to enhance visualization of the monomers; most of the monomers do not fluoresce at 254 nm, and their optical absorbance at that wavelength was too low to provide clear images of their diffusion patterns without the silica plate underneath. The polyethylene film was used to avoid water migration from the gel to the silica. Images were obtained under an ultraviolet (UV) lamp at 254 nm (8 W; VL-4.LC, LTF Labortechnik, Wasserburg/B, Germany) in a darkroom using a Coolpix P1 8MP camera (Nikon, Tokyo, Japan).

Schematic representation of the experimental set-up used for image capturing. The UV light emitted from the lamp passes through the agarose gel and the transparent film to the silica gel. The light reflected from the silica gel is absorbed by the monomers, and the monomers are detected as dark spots on a bright background.

In additional tests, the order of the monomers in the wells was changed to control for any effects of neighboring samples on monomer migration. The monomers were chosen to include hydrophilic neutral monomers commonly used in dental adhesives (i.e. Bis-GMA and TEGDMA), a neutral hydrophilic monomer used in adhesive blends (i.e. HEMA) and two acid hydrophilic monomers used in adhesives (2-MP and TCDM). If any of the neutral monomers migrated in the electric field, it would provide evidence of electroendosmosis (EEO) under those conditions. Only the ionic acidic monomers should migrate toward the anode if they were dissociated.

2.1

Reagents

Bis-GMA (2,2-bis[4-(2-hydroxy-3-methacryloyloxy propoxy) phenyl] propane), HEMA (2-hydroxyethyl methacrylate), 2-MP (bis[2-(methacryloyloxy) ethyl] phosphate, TCDM di(hydroxyethyl methacrylate) ester of 5-(2,5,-dioxo tetrahydrofurfuryl)-3-methyl-3-cyclohexenyl-1,2-dicarboxylic acid), and TEGDMA (triethylene glycol dimethacrylate) were purchased from Sigma Chemical (St. Louis, MO, USA) and used without further purification ( Table 1 ).

Low-electroendosmosis agarose gel D-1 (EEO = 0.09–0.13 by Weime method; sulfate < 0.14%) with a gelling temperature of 36–39 °C, a melting temperature of 87–89 °C, and a gel strength of 1.200 g/cm ² was purchased from Shelton Scientific Inc (Shelton, CT, USA).

2.2

Experimental procedures

Agarose gel powder (0.5 g) was suspended in 100 mL of aqueous buffer at pH 3.1 (2.1% citric acid/1% sodium citrate), 6.3 (1% citric acid/2.9% sodium citrate), 8.5 (3.8% sodium tetraborate boric acid), or 12.3 (0.4% sodium hydroxide). Each buffer was precisely titrated to its nominal pH with HCl 4 N before use. Each agarose gel suspension was heated at full power in a 500-W microwave oven for 2 min to completely solubilize the agarose, poured into a horizontal 10-well electrophoretic cell (Owl EasyCast Horizontal System B1, Thermo Scientific, Portsmouth, NH, USA), and allowed to cool to room temperature. The final gel dimensions were 9 cm × 11 cm, and electrophoresis system buffer capacity was 600 mL. The tested monomers (bis-GMA, HEMA, 2-MP, TCDM, and TEGDMA) were dissolved in ethanol at 5% (w/w) concentration.

A voltage of 50 or 100 V was applied to the cell electrodes using a DC Power Supply (Apelex PS304 MinipacII, Massy, France), and both current and voltage were monitored during experiment. NaCl was added to the buffer used for electrophoresis to adjust their ionic strength to maintain the same electrical current/intensity ratio for all tests without monomer addition (data not shown). The buffers were adjusted so that the current at 100 V was 100 mA (highest ionic strength), 50 mA, or 25 mA (lowest ionic strength).

The dissolved monomers (10-μL aliquots) were injected into the wells of the gel, and voltage was applied for 30 min. After electric field application, the gel was carefully removed from the electrophoretic cell and placed onto a layer of polyethylene film on top of a silica thin-layer chromatography plate (Sigma Chemical) ( Fig. 1 ). The silica plate was used to enhance visualization of the monomers; most of the monomers do not fluoresce at 254 nm, and their optical absorbance at that wavelength was too low to provide clear images of their diffusion patterns without the silica plate underneath. The polyethylene film was used to avoid water migration from the gel to the silica. Images were obtained under an ultraviolet (UV) lamp at 254 nm (8 W; VL-4.LC, LTF Labortechnik, Wasserburg/B, Germany) in a darkroom using a Coolpix P1 8MP camera (Nikon, Tokyo, Japan).

Schematic representation of the experimental set-up used for image capturing. The UV light emitted from the lamp passes through the agarose gel and the transparent film to the silica gel. The light reflected from the silica gel is absorbed by the monomers, and the monomers are detected as dark spots on a bright background.

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