2.1

Chemicals

TEEGMA, Neopen, DPIC, TPSB and TPP were obtained from Sigma–Aldrich (St. Louis, MO, USA). All chemicals and reagents were of the highest purity available. All substances are dissolved in dimethyl sulphoxide (DMSO, 99% purity; Merck, Darmstadt, Germany) and diluted with medium (final DMSO concentration: 1%). Control cells received either DMSO 1% in medium, or 1 mM hydrogen peroxide (H ₂ O ₂ ; VWR International, Darmstadt, Germany).

2.2

Cell culture and drug treatment

HGFs (Cat. No.: 1210412) were obtained from Provitro, Cell-Lining (Berlin, Germany). The HGFs (passage 9) were grown on 175 cm ² cell culture flasks to approximately 75–85% confluence and maintained in an incubator with 5% CO ₂ atmosphere at 100% humidity and 37 °C. Quantum 333 medium supplemented with l -glutamine and 1% antibiotic/antimycotic solution (10,000 U/ml penicillin, 25 mg/ml streptomycin sulphate, 25 mg/ml amphotericin B; PAA Laboratories, Cölbe, Germany) was used to culture HGFs. After reaching confluence, the cells were washed with Dulbecco’s phosphate buffered saline (PAA Laboratories) detached from the flasks by a brief treatment with trypsin/EDTA (PAA Laboratories).

2.3

XTT-based viability assay

Tetrazolium salt XTT (sodium 30-[1-(phenylaminocarbonyl)-3,4-tetrazolium]-bis(4-methoxy-6-nitro) benzene sulfonic acid hydrate) based cell viability assay was used, according to the method described in earlier studies , to determine the half-maximum effect concentrations (EC ₅₀ ) for the tested compounds TEEGDMA, Neopen, DPIC, TPSB and TPP in HGFs and for the estimation of the substance concentrations for the use in the γ-H2AX-assay. HGFs at 20,000 cell/well were seeded into a 96-well microtiter plate in 0.1 ml medium, and then the cells were incubated for 24 h. Then the cells were treated with medium containing DPIC (0.1–30 mM), Neopen (0.1–10 mM), TPSB (0.1–30 mM), TPP (0.1–30 mM), or TEEGDMA (0.1–30 mM). Negative control cells received either medium alone, or medium + DMSO (final DMSO concentration: 1%). Positive control cells received 1% Triton X-100 (Sigma–Aldrich). After incubation for 20 h, the cell monolayer was washed and a mixture of XTT labeling reagent, in RPMI 1640, without phenol red and electron-coupling reagent (PMS [N-methyldibenzopyrazine methyl sulphate] in phosphate buffered saline) was added as recommended by the supplier (cell proliferation kit II; Roche Diagnostics Penzberg, Germany) 4 h before photometric analysis.

The formazan formation was quantified spectrophotometrically at 450 nm (reference wavelength 670 nm) using a micro-titer plate reader (Victor 3, Perkin Elmer Las, Jügesheim, Germany). All experiments were repeated five times.

2.4

γ-H2AX immunofluorescence

DNA-DSBs formation was tested in HGFs unexposed and exposed to TEEGDMA, Neopen, DPIC, TPSB, and TPP by the method of γ-H2AX focus assay. For this microscopic assay, 12 mm round cover slips (Carl Roth, Karlsruhe, Germany) were cleaned in 1 N HCl and distributed into a 24-well plate. In each well medium, HGFs were seeded at 7 × 10 ⁴ cell/ml and followed by overnight incubation at 37 °C. HGFs were exposed to medium containing substances in the following concentrations (mM, corresponding to EC ₅₀ , 1/3 EC ₅₀ and 1/10 EC ₅₀ values, received from the XTT assay): TEEGDMA (4.1, 1.4, 0.41), Neopen (1.1, 0.367, 0.11), DPIC (0.9, 0.3, 0.09), TPSB (1.8, 0.6, 1.8) and TPP (2.4, 0.8, 0.24) for 6 h. Negative controls received either medium alone, or medium + DMSO (final DMSO concentration: 1%). Positive controls received 1 mM H ₂ O ₂ + medium, or 1 mM H ₂ O ₂ + medium + DMSO (final DMSO concentration: 1%) for 10 min. For immunofluorescent staining, cells were first washed 2 × 5 min with PBS, fixed by adding 0.5 ml ice-cold 4% paraformaldehyde in PBS for 5 min at 4 °C, then washed with cold PBS (4 °C) for 4 × 2 min, and permeabilized for 15 min with 0.5 ml of triton-citrate buffer (0.1% sodium citrate, 0.1% Triton X-100) at 4 °C. After washing 4 × 2 min with PBS, cells were blocked for 20 min with 0.2 ml of serum-free blocking buffer (Dako, Hamburg, Germany) per well at 25 °C. Thereafter, cells were incubated with mouse monoclonal anti γ-H2AX (Millipore, Billerica, MA, USA) at 1:1300 dilution in antibody diluent (0.3 ml per well) (Dako) at 4 °C overnight. After 4 × 5 min washes with PBS at 4 °C, cells were incubated with FluoroLink Cy3-labeled goat anti-mouse secondary antibody (GE Healthcare, Munich, Germany) at a dilution of 1:1300 in antibody diluent (0.3 ml per well) for 1 h at 25 °C in the dark. HGFs were then washed 2 × 5 min in PBS, and rinsed 5 min with deionised water at 25 °C. Finally, the cover slips were each placed on 0.2 ml of a mixture of 2 ml Prolong antifade and DAPI (Invitrogen) (76 × 26 mm; Carl Roth, Invitrogen, Karlsruhe, Germany) on a glass slide.

2.5

Apoptosis and necrosis

Apoptosis and necrosis found at EC ₅₀ concentrations of TEEGDMA, Neopen, DPIC, TPSB, and TPP were visually tested in HGFs, exposed to the substances, using the method of γ-H2AX focus assay by the same investigator by eye down the fluorescent microscope. The morphological changes (monitored under microscope) associated with necrosis, which represents cell membrane rupture and lysis of the organized cell structure. Apoptosis represents fragmentation of the cytoplasm and nucleus in the target cell while the normal organelle structure is maintained ( Figs. 6 and 7 ).

2.6

Image acquisition

HGFs were investigated using a Zeiss Axioplan 2 imaging fluorescence microscope (Zeiss, Göttingen, Germany) equipped with a motorized filter wheel and appropriate filters for excitation of red, green and blue fluorescence. Images were obtained using a 63× and a 100× Plan-Neofluar oil immersion objective (Zeiss) and the ISIS fluorescence imaging system (MetaSystems, Altlussheim, Germany).

2.7

Data analysis

2.7.1

XTT test

The values performed from the XTT-based viability assay were calculated as percentage of the 100% control values, using Graph Pad Prism 4 (Graph Pad Software Inc., San Diego, USA), where they were plotted on a concentration log-scale and range of the maximum slope were comprised. Half-maximum-effect substance concentration at the maximum slope was revealed as EC ₅₀ . The EC ₅₀ values were obtained as half-maximum-effect concentrations from the fitted curves. Data are presented as means ± standard error of the mean (SEM). Each experiment was repeated five times. The statistical significance ( p < 0.05) of the differences between the experimental groups was checked using the Student’s t -test, corrected according to Bonferroni–Holm .

2.8

γ-H2AX test

For quantitative analysis of the γ-H2AX test, DSBs (foci) were counted by the same investigator by eye down using the fluorescence microscope (100× objective). Disrupted cells were excluded from the analysis. Cell counting was performed until at least 80 cells were reached, as described in previous study . Each experiment was repeated 3 times. The mean number of cells was scored and the standard error of the mean was calculated. Values were compared using the Student’s t -test ( p < 0.05), corrected according to Bonferroni–Holm. . If one cell contains 40 or more foci, it will be counted as multi-foci cell .

2.9

Statistical analysis of apoptotic and necrotic cells

Apoptotic and necrotic HGF cells were counted using the fluorescence microscope (100× objective). Disrupted cells were excluded from the analysis. Cell counting was performed within 80 cells. Each experiment was repeated 3 times. The mean number of apoptotic and necrotic cells was scored and the standard error of the mean was calculated. The statistical significance ( p < 0.05) of the differences between the experimental groups was compared using the Student’s t -test, corrected according to Bonferroni–Holm .

2.1

Chemicals

TEEGMA, Neopen, DPIC, TPSB and TPP were obtained from Sigma–Aldrich (St. Louis, MO, USA). All chemicals and reagents were of the highest purity available. All substances are dissolved in dimethyl sulphoxide (DMSO, 99% purity; Merck, Darmstadt, Germany) and diluted with medium (final DMSO concentration: 1%). Control cells received either DMSO 1% in medium, or 1 mM hydrogen peroxide (H ₂ O ₂ ; VWR International, Darmstadt, Germany).

2.2

Cell culture and drug treatment

HGFs (Cat. No.: 1210412) were obtained from Provitro, Cell-Lining (Berlin, Germany). The HGFs (passage 9) were grown on 175 cm ² cell culture flasks to approximately 75–85% confluence and maintained in an incubator with 5% CO ₂ atmosphere at 100% humidity and 37 °C. Quantum 333 medium supplemented with l -glutamine and 1% antibiotic/antimycotic solution (10,000 U/ml penicillin, 25 mg/ml streptomycin sulphate, 25 mg/ml amphotericin B; PAA Laboratories, Cölbe, Germany) was used to culture HGFs. After reaching confluence, the cells were washed with Dulbecco’s phosphate buffered saline (PAA Laboratories) detached from the flasks by a brief treatment with trypsin/EDTA (PAA Laboratories).

2.3

XTT-based viability assay

Tetrazolium salt XTT (sodium 30-[1-(phenylaminocarbonyl)-3,4-tetrazolium]-bis(4-methoxy-6-nitro) benzene sulfonic acid hydrate) based cell viability assay was used, according to the method described in earlier studies , to determine the half-maximum effect concentrations (EC ₅₀ ) for the tested compounds TEEGDMA, Neopen, DPIC, TPSB and TPP in HGFs and for the estimation of the substance concentrations for the use in the γ-H2AX-assay. HGFs at 20,000 cell/well were seeded into a 96-well microtiter plate in 0.1 ml medium, and then the cells were incubated for 24 h. Then the cells were treated with medium containing DPIC (0.1–30 mM), Neopen (0.1–10 mM), TPSB (0.1–30 mM), TPP (0.1–30 mM), or TEEGDMA (0.1–30 mM). Negative control cells received either medium alone, or medium + DMSO (final DMSO concentration: 1%). Positive control cells received 1% Triton X-100 (Sigma–Aldrich). After incubation for 20 h, the cell monolayer was washed and a mixture of XTT labeling reagent, in RPMI 1640, without phenol red and electron-coupling reagent (PMS [N-methyldibenzopyrazine methyl sulphate] in phosphate buffered saline) was added as recommended by the supplier (cell proliferation kit II; Roche Diagnostics Penzberg, Germany) 4 h before photometric analysis.

The formazan formation was quantified spectrophotometrically at 450 nm (reference wavelength 670 nm) using a micro-titer plate reader (Victor 3, Perkin Elmer Las, Jügesheim, Germany). All experiments were repeated five times.

2.4

γ-H2AX immunofluorescence

DNA-DSBs formation was tested in HGFs unexposed and exposed to TEEGDMA, Neopen, DPIC, TPSB, and TPP by the method of γ-H2AX focus assay. For this microscopic assay, 12 mm round cover slips (Carl Roth, Karlsruhe, Germany) were cleaned in 1 N HCl and distributed into a 24-well plate. In each well medium, HGFs were seeded at 7 × 10 ⁴ cell/ml and followed by overnight incubation at 37 °C. HGFs were exposed to medium containing substances in the following concentrations (mM, corresponding to EC ₅₀ , 1/3 EC ₅₀ and 1/10 EC ₅₀ values, received from the XTT assay): TEEGDMA (4.1, 1.4, 0.41), Neopen (1.1, 0.367, 0.11), DPIC (0.9, 0.3, 0.09), TPSB (1.8, 0.6, 1.8) and TPP (2.4, 0.8, 0.24) for 6 h. Negative controls received either medium alone, or medium + DMSO (final DMSO concentration: 1%). Positive controls received 1 mM H ₂ O ₂ + medium, or 1 mM H ₂ O ₂ + medium + DMSO (final DMSO concentration: 1%) for 10 min. For immunofluorescent staining, cells were first washed 2 × 5 min with PBS, fixed by adding 0.5 ml ice-cold 4% paraformaldehyde in PBS for 5 min at 4 °C, then washed with cold PBS (4 °C) for 4 × 2 min, and permeabilized for 15 min with 0.5 ml of triton-citrate buffer (0.1% sodium citrate, 0.1% Triton X-100) at 4 °C. After washing 4 × 2 min with PBS, cells were blocked for 20 min with 0.2 ml of serum-free blocking buffer (Dako, Hamburg, Germany) per well at 25 °C. Thereafter, cells were incubated with mouse monoclonal anti γ-H2AX (Millipore, Billerica, MA, USA) at 1:1300 dilution in antibody diluent (0.3 ml per well) (Dako) at 4 °C overnight. After 4 × 5 min washes with PBS at 4 °C, cells were incubated with FluoroLink Cy3-labeled goat anti-mouse secondary antibody (GE Healthcare, Munich, Germany) at a dilution of 1:1300 in antibody diluent (0.3 ml per well) for 1 h at 25 °C in the dark. HGFs were then washed 2 × 5 min in PBS, and rinsed 5 min with deionised water at 25 °C. Finally, the cover slips were each placed on 0.2 ml of a mixture of 2 ml Prolong antifade and DAPI (Invitrogen) (76 × 26 mm; Carl Roth, Invitrogen, Karlsruhe, Germany) on a glass slide.

2.5

Apoptosis and necrosis

Apoptosis and necrosis found at EC ₅₀ concentrations of TEEGDMA, Neopen, DPIC, TPSB, and TPP were visually tested in HGFs, exposed to the substances, using the method of γ-H2AX focus assay by the same investigator by eye down the fluorescent microscope. The morphological changes (monitored under microscope) associated with necrosis, which represents cell membrane rupture and lysis of the organized cell structure. Apoptosis represents fragmentation of the cytoplasm and nucleus in the target cell while the normal organelle structure is maintained ( Figs. 6 and 7 ).

2.6

Image acquisition

HGFs were investigated using a Zeiss Axioplan 2 imaging fluorescence microscope (Zeiss, Göttingen, Germany) equipped with a motorized filter wheel and appropriate filters for excitation of red, green and blue fluorescence. Images were obtained using a 63× and a 100× Plan-Neofluar oil immersion objective (Zeiss) and the ISIS fluorescence imaging system (MetaSystems, Altlussheim, Germany).

2.7

Data analysis

2.7.1

XTT test

The values performed from the XTT-based viability assay were calculated as percentage of the 100% control values, using Graph Pad Prism 4 (Graph Pad Software Inc., San Diego, USA), where they were plotted on a concentration log-scale and range of the maximum slope were comprised. Half-maximum-effect substance concentration at the maximum slope was revealed as EC ₅₀ . The EC ₅₀ values were obtained as half-maximum-effect concentrations from the fitted curves. Data are presented as means ± standard error of the mean (SEM). Each experiment was repeated five times. The statistical significance ( p < 0.05) of the differences between the experimental groups was checked using the Student’s t -test, corrected according to Bonferroni–Holm .

2.8

γ-H2AX test

For quantitative analysis of the γ-H2AX test, DSBs (foci) were counted by the same investigator by eye down using the fluorescence microscope (100× objective). Disrupted cells were excluded from the analysis. Cell counting was performed until at least 80 cells were reached, as described in previous study . Each experiment was repeated 3 times. The mean number of cells was scored and the standard error of the mean was calculated. Values were compared using the Student’s t -test ( p < 0.05), corrected according to Bonferroni–Holm. . If one cell contains 40 or more foci, it will be counted as multi-foci cell .

2.9

Statistical analysis of apoptotic and necrotic cells

Apoptotic and necrotic HGF cells were counted using the fluorescence microscope (100× objective). Disrupted cells were excluded from the analysis. Cell counting was performed within 80 cells. Each experiment was repeated 3 times. The mean number of apoptotic and necrotic cells was scored and the standard error of the mean was calculated. The statistical significance ( p < 0.05) of the differences between the experimental groups was compared using the Student’s t -test, corrected according to Bonferroni–Holm .