AGE was prepared as previously described (12). Briefly, AGE was manufactured according to the following steps: Originally grown raw garlic (A sativum L.) was cut into slices, immersed in aqueous ethanol, and extracted for >10 months at room temperature (12). The sulfur-containing amino acids, S1PC, SAC and SAMC, are produced during the aging process of raw garlic in 50% ethanol solution for >10 months (19). The purification and structure determination of sulfur compounds in AGE was performed by high performance liquid chromatography (HPLC) and liquid chromatography-mass spectrometry (LC-MS) systems as previously described (9).

Dulbecco's modified Eagle's medium (DMEM, D6046) and WST-1 reagent (501594401) were purchased from Sigma-Aldrich. Fetal bovine serum (FBS, 10270), 0.05% trypsin/EDTA solution (25300-054), Halt protease and phosphatase inhibitor single-use cocktail (1861280) and TRIzol reagent (15596018) were from Thermo Fisher Scientific. Penicillin/streptomycin (164-25251) and recombinant human TNF-α (207-15261) were from Wako Pure Chemical Industries. Human β-defensin-3 (hβD3, 4382-s) was from Peptide Institute Inc. Anti-intercellular adhesion molecule-1 (ICAM-1) (4915S), anti-phosphorylated nuclear factor κ-light-chain-enhancer of activated B cells (NF-κB) p65 (3033) antibodies and a horseradish peroxidase (HRP)-conjugated rabbit immunoglobulin G (IgG) (7074S) were from Cell Signaling Technologies. An anti-NF-κB p65 antibody (sc-109X) was from Santa Cruz Biotechnology. RIPA lysis buffer (20-188) was purchased from Merck Millipore. An HRP-conjugated anti-β-actin antibody (PM053-7) was from MBL Life Science.

The human gingival epithelial cells, Ca9-22 (JCRB0625, Lot. 11182016, Biomedical Innovation, Health and Nutrition Research Institute) were cultured in DMEM containing 10% fetal bovine serum, 100,000 units/ml penicillin and 100 µg/ml streptomycin in 5% CO₂ at 37˚C. The Ca9-22 cells were subcultured 2 or 3 times per week. For pharmacological experiments, the cells were seeded onto a 6- or 12-well plate at the density of 1 to 2x10⁵ cells per well and cultured for 36 to 48 h. When they reached full confluency, the cells were treated with TNF-α (100 ng/ml) in the absence or presence of AGE (0.01-1 mg/ml), S1PC, SAC and SAMC (each at 1 to 100 µM) for the 3, 6, 12 or 24 h. In the experiment with cycloheximide (CHX, Fig. 4), the cells were pre-treated with TNF-α (100 ng/ml) for 12 h, and then treated with S1PC (10 µM) in the absence or presence of CHX (10 µM) for 6 h.

Following treatment of the cells with TNF-α (100 ng/ml) in the absence or presence of AGE (0.01-1 mg/ml), S1PC, SAC or SAMC (each at 1 to 100 µM) for 6 h, an aliquot of culture medium was collected and frozen at -80˚C until use. The IL-6 protein amount in the medium was determined with a human IL-6 Uncoated enzyme-linked immunosorbent assay (ELISA) kit (88-7066-22, Thermo Fisher Scientific).

Cells were washed with phosphate-buffered saline (PBS) 5 times and total protein was extracted with RIPA lysis buffer containing protease inhibitor cocktail. The protein amount in the extract was determined with the Pierce BCA Protein Assay kit (23225, Thermo Fisher Scientific) with bovine serum albumin (BSA, A7030, Sigma) as a standard. The protein extract (10 µg) was denatured by the addition of sample buffer [5% sodium dodecyl sulfate, 12.5% glycerol and 50 mM dithiothreitol in 100 mM Tris-hydrochloric acid (HCl) buffer, pH 6.8], and was heated at 95˚C for 5 min. The samples were separated by electrophoresis and were blotted onto a nitrocellulose membrane (1620090, Bio-Rad). The blotted membrane was blocked with 5% non-fat dry milk (999S, Cell Signaling Technology) in Tris-buffered saline (TBS)-T buffer (0.1% Tween-20, pH 7.6) for 1 h, and was subsequently incubated in the presence of the rabbit anti-ICAM-1 (4915S, Cell Signaling Technology), anti-NF-κB (sc-109X, Santa Cruz Biotechnology) or anti-phosphorylated NF-κB (3033, Cell Signaling Technology) antibody at a 1:2,000 dilution overnight at 4˚C. The membrane was washed 3 times and incubated in the presence of the HRP-conjugated anti-rabbit IgG antibody (7074S, Cell Signaling Technology) for 1 h at room temperature. On the other hand, another blotted membrane was incubated with the HRP-conjugated anti-β-actin antibody (PM053-7, MBL Life science) at a 1:2,000 dilution for 1 h at room temperature, in order to quantitatively normalize the immunoreactive ICAM-1 protein levels. After washing, immunoreactive proteins on the nitrocellulose membrane were visualized with Armasham ECL Prime peroxidase solution (RPN2232V, GE Healthcare), by using a luminoimage analyzer (ChemiDoc^™ MP, Bio-Rad). The density of each immunoreactive band was analyzed with Image Lab^™ software ver. 4.1 (Bio-Rad).

Total RNA was isolated from cells with TRIzol reagent. Contaminated genomic DNA in the total RNA was removed by incubation with gDNA eraser (RR047A, Takara) for 5 min at room temperature, and total RNA was reverse transcribed into complementary DNA (cDNA) with a PrimeScript RT reagent kit with genomic DNA Eraser (RR047A, Takara). cDNA was amplified with primer pairs using a SYBR Premix Ex Taq II (RR820A, Takara). The level of gene expression relative to the internal control (β-actin) was calculated by performing a quantitative (real-time) PCR with a Real-time PCR system (PikoReal 96, Life Technologies; Thermo Fisher Scientific). The reaction was run using the following program: 30 sec at 95˚C, 40 repeats of 10 sec at 95˚C, 10 sec of 63˚C and 15 sec of 72˚C. The sequences of the specific primers were as follows: human ICAM-1 forward, 5'-TCGGCACAAAAGCACTATATG-3' and reverse, 5'-ACAGGACAAGAGGACAAGGC-3'; human IL-6 forward, 5'-TCTCCACAAGCGCCTT-3' and reverse, 5'-CTCAGGGCTGAGATGC-3'; and β-actin forward, 5'-CGCGAGAAGATGACCCAGAT-3' and reverse, 5'-GGTGAGGATCTTCATGAGGTAGTC-3'. The fold change in the relative mRNA level to β-actin was calculated based on the Cq (ΔΔCq) method (20).

Following treatment of the cells with TNF-α (100 ng/ml) in the absence or presence of AGE (1 mg/ml) or SAC (100 µM) for 3 h, the total protein was extracted with RIPA buffer. The amount of IL-6 protein in the extract was determined by ELISA, as described above. The cellular IL-6 protein content is expressed relative to 1 mg total protein.

Data are expressed as the means ± standard deviation (SD). Statistical significance was evaluated using the Student's t-test for differences between 2 groups or one-way analysis of variance (ANOVA), followed by Tukey's post hoc test for differences between >3 groups. A P-value <0.05 was statistically significant in comparison to control or the effect of TNF-α alone.

Human gingival fibroblasts and Ca9-22 cells have been shown to express ICAM-1 in response to the periodontal disease bacteria, P.g.-derived LPS or TNF-α (21-25). It was also found that ICAM-1 protein expression in the Ca9-22 cells was profoundly induced by treatment with TNF-α in a concentration-dependent manner (Fig. 1A). In addition, the ICAM-1 protein level began to increase at 3 h, reached peak levels at 12 h and remained elevated until 24 h (Fig. 1B). As shown in Fig. 1C, the presence of S1PC for 24 h inhibited the increased level of TNF-α-induced ICAM-1 protein in a concentration-dependent manner, whereas treatment with AGE exerted minimal inhibitory effects even at the highest concentration (1 mg/ml) (Fig. 1D). Both SAC and SAMC also had no significant effect (Fig. 1E and F).

It has been previously demonstrated that the anti-microbial peptide hβD3 reduces the level of TNF-α-elicited ICAM-1 protein in human vein endothelial cells (HUVECs) (26). Thus, this study examined whether the peptide inhibits the level of ICAM-1 protein in Ca9-22 cells. As shown in Fig. 1G, the increased level of TNF-α-induced ICAM-1 protein was moderately but significantly suppressed by hβD3 at 10 nM, indicating that this peptide is also effective. Furthermore, it was found that the inhibitory effect of hβD3 was enhanced by simultaneously treating the cells in the presence of S1PC (Fig. 2), suggesting the synergistic effect of hβD3 and S1PC.

It is conceivable that the inhibitory effect of S1PC on the level of ICAM-1 protein was due to the suppression of ICAM-1 gene transcriptions. Thus, this study then examined the effects of S1PC as well as those of hβD3 over a period of 3 or 24 h treatment on the TNF-α-induced ICAM-1 gene expression by RT-qPCR. As shown in Fig. 3A, TNF-α significantly enhanced the basal ICAM-1 mRNA transcription level with a peak at 3 h. Treatment with S1PC or hbD3 for either 3 or 24 h had no effect on the mRNA expression level of ICAM-1 increased by TNF-α (Fig. 3B and C). These results suggested that the actions of S1PC and hβD3 occurred at the post-transcriptional level, since these compounds did not affect ICAM-1 expression even at the concentrations at which induced a decrease in the protein level.

Since S1PC did not affect ICAM-1 gene expression, we then examined their effect at the translational level using CHX, an inhibitor of protein synthesis. As shown in Fig. 4, the inhibitory effects of CHX on the protein level of ICAM-1 were enhanced in the presence of S1PC in cells treated with TNF-α. This result suggested that the effects of S1PC occurred at the post-translational level, since this compound induced a further reduction in the ICAM-1 protein level when total protein synthesis was blocked.

IL-6 is produced in human gingival epithelial cells in response to LPS or TNF-α, leading to the activation of osteoclasts via the upregulation of receptor activator of NF-κB ligand (RANKL) in osteoblasts (21). This study thus examined the effects of TNF-α on IL-6 secretion in Ca9-22 cells. As shown in Fig. 5A, TNF-α stimulated basal IL-6 secretion during 6 h of culture. The enhanced IL-6 secretion induced by TNF-α was reduced by simultaneous treatment with AGE, SAC or SAMC in a concentration-dependent manner (Fig. 5A-C). On the other hand, S1PC had no effect on IL-6 secretion even at the concentration of 100 µM (Fig. 5D).

It was possible that SAC and SAMC downregulated IL-6 gene transcription induced by TNF-α. Thus, the effectσ of these sulfur compounds on the IL-6 gene expression level were then examined by RT-qPCR. It was found that TNF-α significantly enhanced the basal IL-6 mRNA transcription level with a peak at 3 h (Fig. 6A). As shown in Fig. 6B-D, treatment with AGE, SAC or SAMC for 3 h had a minimal effect on the enhanced IL-6 mRNA expression level induced by TNF-α.

In order to examine whether AGE and sulfur compounds affect the IL-6 secretion process, the cellular IL-6 protein content was measured during TNF-α stimulation by ELISA. Treatment with AGE (1 mg/ml) or SAC (100 µM) for 3 h exhibited a tendency to enhance the effects of TNF-α on the cellular IL-6 content, although their effects were not statistically significant (Fig. 7).

Stimulation of the cells with TNF-α has been shown to activate a variety of signaling pathways and transcription factors, such as NF-κB, which plays an essential role in the expression of inflammation-related molecules (26-28). In addition, hβD3 has been shown to alleviate periodontitis via the suppression of NF-κB (29). Thus, this study examined the effects of hβD3, S1PC, AGE, SAC and SAMC on the phosphorylation (activation) of NF-κB induced by TNF-α. As shown in Fig. 8A and C-E, hβD3 (100 nM), AGE (1 mg/ml), SAC and SAMC (each at 100 µM) inhibited NF-κB activation, whereas S1PC (100 µM) did not have any significant effect (Fig. 8B).