Background
The oral cavity is a suitable milieu for bacterial growth and propagation. The presence of bacteria in the mouth readily stimulates the formation of dental plaque, which accumulates on both hard and soft tissues as dental calculus. Although the regional colonization and invasion of bacteria are rigorously controlled by the dynamic equilibrium between dental plaque bacteria (DPB) and the host’s innate defense mechanisms [
1], plaque that extends subgingivally can trigger the immune system imbalance, inducing an inflammatory response [
2]. Gingivitis and periodontitis are the most common plaque-induced inflammatory conditions.
Aggregatibacter actinomycetemcomitans,
Porphyromonas gingivalis,
Prevotella intermedia, and
Tannerella forsythensis are the most prevalent anaerobic gram-negative bacteria in subgingival area. All are critical in the onset and subsequent development of periodontitis. If untreated, these bacteria can lead to the periodontal pocket, connective tissue destruction, and alveolar bone resorption [
3].
Bacteria involved in the initiation and progression of periodontal disease are classified into color-coded groups. The categories are based upon the pathogenicity of the bacteria and their role in the development of plaque [
4]. Species in the red complex (
P. gingivalis,
T. forsythia, and
Treponema denticola) are strongly related with pocket depth and bleeding on probing. The red complex can be used as a clinical parameters that is considered the most meaningful in periodontal diagnosis. Species in the orange complex (
Fusobacterium nucleatum,
P. intermedia,
Prevotella nigrescens,
Peptostreptococcus micros,
Streptococcus constellatus,
Eubacterium nodatum, and
Campylobacter gracilis) are closely associated with one another. The orange complex is closely related to the red complex. Similarly to the red complex, the orange complex is significantly associated with increasing pocket depth; a decreased level of these species lead to improvement in periodontal status.
A. actinomycetemcomitans, which is classified in the green complex, is associated with localized aggressive periodontitis.
Toxins produced by DPB, such as lipopolysaccharide (LPS), stimulate an inflammatory response. LPS induces the release of various inflammatory mediators from gingival tissue, which activates the innate immune system of the host to eliminate the inflammation [
5]. Although such mediators are normally part of a beneficial host response to suppress bacterial proliferation, they can also damage the area of inflammation. During the inflammatory-immune response in gingivitis and periodontitis, inflammatory cytokines and matrix metalloproteinases (MMPs) are produced, which destroy the extracellular matrix (ECM) and lead to periodontal bone loss [
6]. In periodontal disease, the irreversible breakdown of collagen fibers in the periodontal ligament results in tissue destruction.
Epidemiological studies have consistently revealed the increase risk for periodontal disease with age. The National Health and Nutrition Examination Survey (NHANES) recently estimated that in the United States 47.2% of adults 30 years of age and older have periodontitis [
7], and the prevalence of periodontitis among all adults increases with increasing age. The fact that over the past 2 years the risk of periodontitis has increased approximately 53.0% indicates the need for more intensive oral hygiene and dental care, and the dissemination of information regarding the treatment and prevention of periodontal disease [
8].
The properties of various extracts of the fruit of the
Terminalia chebula tree have been widely investigated and include anti-diabetic, anti-mutagenic, anti-oxidant, anti-bacterial, anti-fungal, and anti-viral effects [
9]. Many of these beneficial effects are related to the presence of various phytochemicals including polyphenols, terpenes, anthocyanins, flavonoids, alkaloids, and glycosides [
10]. In the present study, we determined the effects of an ethanol extract of
T. chebula (EETC) in preventing DPB-induced inflammation and bone resorption, and identified the principal molecules in this inflammatory response that are regulated by EETC. The data indicate the potential value of EETC in preventing DPB-mediated periodontal disease.
Methods
Materials and reagents
Minimum essential medium alpha medium (α-MEM), RPMI 1640 medium, Dulbecco’s modified Eagle’s medium (DMEM)/F-12 phenol red-free medium (1:1), fetal bovine serum (FBS), antibiotic-antimycotic mixture (100×), phosphate-buffered saline (PBS), and 0.25% trypsin-EDTA (1×) were purchased from Gibco BRL Co. (Grand Island, NY). Dimethyl sulfoxide (DMSO), LPS, and 3-(4,5 dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) were obtained from Sigma-Aldrich (St Louis, MO). Recombinant mouse soluble RANK ligand (sRANKL) was purchased from Koma Biotech (Seoul, Republic of Korea). Recombinant mouse macrophage colony-stimulating factor (M-CSF) was purchased from R&D System (Minneapolis, MN). EETC was provided by COSMAX Inc. R&I Center (Seongnam City, Republic of Korea).
Plant material
T. chebula fruit were collected from southwest China (Yunnan province) in 2014. Taxonomic identification was done by a botanist and herbalist at COSMAX. A voucher specimen (CH209) was deposited in the COSMAX Inc. R&I Center.
T. chebula fruit were thoroughly washed with distilled water to remove dirt and soil, and dried under shade and ventilation. The dried fruits were ground using an electronic miller. The powder was extracted using 70% ethanol for 72 h at room temperature, filtered through Whatman filter paper No. 1, and concentrated using a rotary evaporator under reduced pressure. The dried extracts were stored in a refrigerator until for further use. Stock solution was aliquoted and stored frozen at −70 °C for up to 6 months. Freeze/thaw cycles were avoided.
Bacterial culture and preparation
Streptococcus mutans, Aggregatibacter actinomycetemcomitans, and DPB were cultured in brain-heart infusion (BHI) broth (Becton, Dickinson and Company, Baltimore, MD) at 37 °C with shaking at 200 rpm. Dental plaques were obtained through regular scaling from a participant without any oral mucosal disease and all procedures were performed by dental hygienist. Informed consent was given by the participant. Cells were harvested and PBS-washed three times by centrifugation at 3,000 rpm for 5 min. The washed cells were suspended in PBS and absorbance was measured at 600 nm using a DU 800 spectrophotometer (Beckman Coulter, Palo Alto, CA). A standard curves was generated for each bacterial sample and colony forming units (CFU)/ml was determined. For experiments requiring plate cultures, a bacterial suspension was subcultured onto the surface of BHI agar and bacterial growth was assessed. To stimulate the cultured cells, a multiplicity of infection (MOI) of 200 bacteria was applied for 24 h at 37 °C and 5% CO2.
Minimum inhibitory concentrations (MICs) assay
MICs were determined for the EETC by the broth dilution method after incubation at 37 °C for 24 h under 5% CO2, with each determination done in triplicate. A MIC was the lowest concentration of test sample that completely inhibited visible growth in the broth.
LPS was extracted using a LPS extraction kit (iNtRON Biotechnology, Seongnam City, Republic of Korea) according to the manufacturer’s protocol. DPBs samples (DPB#1, DPB#2, or DPB#3) were harvested when the culture was at an optical density at 600 nm (OD600) of 0.8 to 1.2. Lysis and purification buffers were sequentially applied, and the LPS pellet was dissolved by boiling for 3 min. LPS was quantified using the Limulus Amebocyte Lysate Chromogenic Endotoxin Quantitation Kit (Pierce Biotechnology, Rockford, IL) according to the manufacturer’s protocol. Escherichia coli O111:B4 was used as the standard of known concentration. Ten endotoxin units (EU)/mL equaled approximately 1 ng/ml.
RAW264.7 macrophage cells were cultured in RPMI 1640 containing 10% FBS and 1% antibiotic-antimycotic mixture at 37 °C and 5% CO
2. Human fetal osteoblastic cells (hFOB1.19; American Type Culture Collection, Manassas, VA) were cultured in DMEM/F-12 containing 10% FBS and 1% antibiotic-antimycotic mixture. Immortalized human oral keratinocytes (IHOK), immortalized human gingival fibroblasts (IGF), and YD38 human gingival epithelial cells were obtained from the Yonsei University College of Dentistry, Republic of Korea, and all were cultured in DMEM/F12 (3:1 ratio) as previous detailed [
11]. Mouse bone marrow-derived macrophages (BMMs) were isolated from the tibias of 4-week-old ICR male mice using Histopaque density gradient centrifugation. BMMs were cultured in α-MEM containing 10% FBS, M-CSF (30 ng/ml), and a 1% antibiotic-antimycotic mixture.
In vitro susceptibility test
In vitro susceptibility was assessed using the disc diffusion method. Briefly, the bacterial suspension in agarose solution was inoculated on BHI agar plates, and the gel was allowed to solidify completely at room temperature. Whatman filter discs with DMSO, ampicillin (Amp, 10 μg/disc), or EETC (5 μg, 10 μg/disc) were placed on the plates and cultured overnight at 37 °C and 5% CO2. Susceptibility was assessed using linear fitting of the squared radius (diameter in mm) of the inhibition zones. Ampicillin was used for comparing the assay results. DMSO (0.01%) was used as the control.
Cytotoxicity assay
Cells (1 × 104 cells/well) were added to wells of a 96-well culture plate. After 24 h, the fluid was replaced with complete medium containing EETC and incubation continued for 24 h. Cell viability was measured by the MTT assay, which is based on the ability of viable cells to convert soluble MTT into an insoluble dark blue formazan. MTT solution (5 mg/ml) was added to each well and the plate was incubated at 37 °C for 4 h. The purple formazan product was dissolved with 200 μl DMSO and the optical density at 570 nm was determined with a microplate reader (Bio-Rad, Hercules, CA).
Prostaglandin E2 (PGE2) assay
Concentration of human PGE2 was measured by an ELISA kit (R&D Systems) according to the manufacturer’s protocol. Cells (1 × 105 cells/well) were cultured in complete medium in wells of a 6-well plate. After being washed with PBS, the cells were exposed to serum-free medium containing LPS (1 μg/ml) and/or EETC (10 mg/ml) for 24 h. The culture medium was collected by centrifugation at 1,500 rpm for 10 min and was examined by ELISA. DPB#1, DPB#2, and DPB#3 were independently co-cultured with RAW264.7 macrophages, IHOK keratinocytes, IGF gingival fibroblasts, YD38 gingival epithelial cells. Cultured media were harvested by centrifugation and used to determine the level of PGE2. LPS extracted from the three DPB samples (DPB#1-LPS, DPB#2-LPS, and DPB#3-LPS) were also treated instead of DPB.
Reverse transcription-polymerase chain reaction (RT-PCR)
Total RNA was isolated using the Trizol (Invitrogen, Carlsbad, CA). Single-stranded cDNA was transcribed from the RNA using Promega’s reverse transcription system (Madison, WI). Then PCR was performed with cDNA in a reaction mixture containing 25 mM magnesium chloride (MgCl2), dNTPs, reverse and forward primers, and Taq polymerase (Takara Bio, Shiga, Japan). The following primers were used for PCR: F-COX2, 5′-ATGACTTCCAAGCTGGCCGT-3′ and R-COX2, 5′-CCTCTTCAAAAACTTCTCCACACC-3′ (annealing temperature; 57 °C, PCR product size; 305 base pair): F-RANKL, 5′-GCCAGTGGGAGATGTTAG-3′ and R-RANKL, 5′-TTAGCTGCAAGTTTTCCC-3′ (annealing temperature; 48 °C, PCR product size; 486 base pair): F-OPG, 5′-GGGGACCACAATGAACAAGTTG-3′ and R-OPG, 5′-AGCTTGCACCACTCCAAATCC-3′ (annealing temperature; 55 °C, PCR product size; 409 base pair): F-GAPDH, 5′-CCCCCTACTGCCCACTGCCACCAC-3′ and R-GAPDH, 5′-TCCATCCACTATGTCAGCAGGTCC-3′ (annealing temperature; 52 °C, PCR product size; 420 base pair). The amplified PCR product was electrophoresed on a 2% agarose gel in 1× Tris-Borate-EDTA buffer containing ethidium bromide and visualized using Quantity One software and the Gel Doc 2000 system (Bio-Rad).
Inflammation antibody array
Inflammatory cytokine profiles were measured using a Human Inflammation Array C3 Kit (RayBiotech, Norcross, GA) according to the manufacturer’s protocol. Briefly, DPB-LPS (1 μg/ml) and/or EETC (10 mg/ml) was added in culture medium and harvested after 24 h treatment for conditioned medium (CM). Cytokine array membranes were blocked with blocking buffer and incubated with equal protein amounts of CM for 24 h. After extensive sequential washing with Buffer I and Buffer II, the membrane was reacted with a cocktail of biotin-conjugated antibodies against different individual cytokines. The membrane were washed again and reacted with horseradish peroxidase (HRP)-conjugated streptavidin. Relative protein expression was detected by the enhanced chemiluminescence (ECL) system. Densitometric values were quantified using TINA-program software.
Protease array
Before application to the array, the protein concentration of the CM was normalized by dilution with serum-free media. Then CM was incubated for 24 h with the Proteome Profiler Human Protease Array Kit (R&D Systems). The relative expression levels of the proteases were determined according to the manufacturer’s protocol, and signal intensities were compared using Quantity One software and the Gel Doc 2000 system (Bio-Rad).
ECM degradation
Fluorescein isothiocyanate (FITC)-conjugated gelatin matrix-coated coverslips were prepared as described previously [
12]. After the coverslips were quenched for 1 h with complete media at 37 °C, the cells were plated and cultured in medium with DPB-LPS (1 μg/ml) and/or EETC (10 mg/ml). Cells were fixed with 4% paraformaldehyde followed by permeabilization with 0.5% Triton X-100/PBS. Dark areas lacking fluorescence on the coverslips were observed with a LSM 510 META confocal laser scanning microscope (Carl Zeiss, Oberkochen, Germany).
Mouse BMMs (5 × 104 cells/well) were plated and cultured in α-MEM complete media containing M-CSF (30 ng/ml), sRANKL (10 ng/ml or 100 ng/ml), DPB-LPS (1 μg/ml), and/or EETC (10 μg/ml) for 7 days with replacement with fresh medium every second day. The cells were fixed with 4% paraformaldehyde for 10 min. Cells were reacted with the Acid Phosphatase, Leukocyte (TRAP) kit (Sigma-Aldrich) according to the manufacturer’s instruction. The number of TRAP-positive multinucleated cells (≥3 nuclei) were counted as osteoclasts per well. Reaction with only M-CSF was performed for control.
Osteo Assay Surface Polystyrene Stripwells (Corning, Corning, NY) were used to observe pit formation as a measure of osteoclast activity. Mouse BMMs (5 × 104 cells/well) were plated on stripwells and cultured in α-MEM complete media containing M-CSF (30 ng/ml), sRANKL (10 ng/ml or 100 ng/ml), DPB-LPS (1 μg/ml), and/or EETC (10 μg/ml). Cultures were fed every 2 days with fresh medium. After a 15-days incubation period, all remaining cells were lysed using 5% sodium hypochlorite solution. Images of the resorbed pits were obtained under light microscopy.
Statistical analysis
The statistical analysis was conducted using InStat™ statistical software (GraphPad Software, San Diego, CA). Data are expressed as mean ± standard errors. Asterisks were used to graphically indicate the statistical significance. The statistical significance of differences between groups was analyzed via repeated measures of one-way ANOVA. P values of <0.05 were considered significant.
Discussion
Inflammation is the biological response of tissues to infection with pathogens and cell damage [
15]. When harmful stimuli cause an inflammatory response, the body’s innate immune system involves the phagocytic activation of leukocytes and macrophages, and the increased release of inflammatory cytokines. Uncontrolled inflammation leads to disease progression because of the excessive production of inflammatory cytokines [
16]. DPB are a leading cause of inflammation in periodontal disease [
17]. Untreated gingivitis readily progresses to periodontitis and leads to tissue destruction. Bacterial plaque elaborate various compounds that elicit an inflammatory response and lead to destruction of the gingival tissue, which may progress to destruction of the periodontal ligaments. Plaque control is required to prevent further progression of inflammation. In this study, we tried to elucidate the critical factors involved in plaque bacteria-induced inflammation and effective natural anti-inflammatory substances for plaque bacteria control.
The in vitro anti-bacterial activity of EETC against DPB was evaluated. Disc diffusion assay results showed that EETC effectively suppressed the DPB growth and the anti-bacterial activity of EETC were increased with increasing concentration of extract. This concentration of EETC was not cytotoxic to gingival epithelial cells, gingival fibroblasts and macrophage. The induction of inflammatory factors and proteases that contributed to the inflammatory reaction were also abolished by EETC. These results indicate that EETC could effectively suppress the inflammatory responses induced by plaque bacteria. The collective data indicate that EETC is useful in reducing bacterial plaque accumulation and gingival inflammation, thereby preventing periodontal disease. Since the efficacy and safety of EETC has been established, it can be developed into a mouthwash without added alcohol. Many commercially available mouthwashes contain alcohol, which increases the risk of oral cancers and dry mouth.
LPS is also known as lipoglycans and endotoxins. The molecules is a component of the outer membrane of the cell wall of gram-negative bacteria, and is one of the most powerful bacterial virulence factors in the pro-inflammatory response [
18]. Initiation of the inflammatory response by LPS stimulates a strong immune response. LPS acts as the prototypical endotoxin through binding to the CD14/TLR4/MD2 receptor complex in many cell types, but especially in monocytes, dendritic cells, macrophages, and B cells, which promotes the secretion of pro-inflammatory cytokines, nitric oxide, and eicosanoids [
19]. Therefore, LPS is a central molecule in the pathogenesis of certain bacterial infections [
20]. In this study,
in vitro co-culture with gingival epithelial cells and plaque bacteria caused pH changes of the culture medium during 24 h of incubation. Therefore, LPS was extracted from DPBs and its capacity to induce inflammation was verified. DPB-LPS significantly increased the levels of inflammatory factors in gingival epithelial cells, gingival fibroblasts and macrophages. EETC also effectively suppressed the levels of DPB-LPS-induced inflammatory factors.
EETC significantly suppressed growth of DPB and DPB-mediated periodontal disease. Antibiotics are used to both treat and prevent bacterial infections [
21]. Antibiotics like penicillin and erythromycin used to be highly effective against many bacterial species and strains. They are now less effective because these organisms have developed increased resistance to the drugs [
22]. Dental plaque, which adheres to the gingival sulcus, consists mainly of bacterial cells, salivary polymers, and bacterial extracellular products. Bacterial LPS stimulates the host cells, including macrophages, fibroblasts, and epithelial cells, which abundantly produce cytokines, thereby triggering a direct or an indirect immune response through inflammatory processes [
23]. The growth of bacterial biofilms increases antibiotic resistance and has been implicated in the etiopathogenesis of gingivitis and periodontal disease by inducing inflammation.
An effective substance is needed that will prevent and treat bacterial plaque-mediated disease by controlling bacterial growth and the inflammatory reaction. The fruits of the
T. chebula, which has been amply verified as being medicinally valuable, has been used to treat cancer, cardiovascular diseases, paralysis, leprosy, ulcers, gout, arthritis, epilepsy, cough, fever, diarrhea, gastroenteritis, skin disorders, urinary tract infection, and wound infections [
10,
24].
T. chebula fruit is also effective in the treatment of bacterial infections [
25,
26]. Clinical trials of
T. chebula fruit extract as a mouthwash preparation have reported reduced plaque accumulation and gingival inflammation [
27,
28]. The present findings provide mechanistic details for these beneficial effects.
Most dental care products exert their antibacterial effects by eliminating oral bacteria. Instead, LPS from other types of bacterial cells, such as
E. coli and
Pseudomonas aeruginosa, have been used to induce the inflammation. Inflammatory events related to DPB-derived endotoxins have not been evaluated as intensively [
29,
30], and the value of anti-microbial dental care products to treat periodontal disease has not been sufficiently verified. Thus, there was a need to simultaneously investigate inflammatory events due to DPB-derived endotoxin and elucidate an effective anti-microbial component for periodontal disease. Here we demonstrate that DPB and DPB- significantly increase inflammation-associated elements such as COX-2 and PGE2. Many inflammatory molecules and proteases are also upregulated by DPB-LPS and lead to matrix damage. In addition, DPB-LPS stimulation promotes osteoclast formation, causing bone resorption. The risk of bone loss tends to increase in patients with inflammatory conditions [
31]. Inflammatory cytokines modulate osteoblast and osteoclast activity [
32]. Interleukins (IL), tumor necrosis factor (TNF), and tumor necrosis factor receptor superfamily members (TNFRSF) perturb bone homeostasis, leading to increased cartilage degradation and bone resorption by osteoclasts and inhibiting bone formation by osteoblasts [
33].
In the present study, IL-3, IL-16, CXCL10, TNFRSF1A, TNFRSF1B, M-CSF 1, and CCL4 were increased in DPB-LPS-stimulated gingival epithelial cells. Proteases including MMP-3, MMP-7, KLK 10, CTSC, and PC9, which were also increased by DPB-LPS stimulation, might also contribute to the inflammatory reaction, thereby leading to matrix degradation and bone destruction. However, the levels of inflammation-related molecules and osteoclastic bone resorption were significantly reduced by treatment with EETC. EETC also exhibited anti-bacterial properties by arresting the growth of DPB. These findings suggest that the EETC could be used to treat DPB-mediated periodontal disease.
Osteoclast differentiation and bone resorption activity require stimulation by the receptor activator of nuclear factor-kappaB (RANKL) expressed on osteoblasts [
34]. In the present study, increased RANKL mRNA expression was observed in DPB-LPS-stimulated hFOB1.19 human osteoblast cells. In addition, DPB-LPS stimulated osteoclast formation and bone resorption under RANKL-limited conditions. These results are consistent with the results of previous studies showing that LPS stimulated osteoclastogenesis [
35‐
37]. These results indicate that DPB-LPS promotes functional osteoclast formation through osteoblast-dependent and osteoblast-independent pathways. DPB-LPS-induced osteoclast formation and bone resorption were also significantly abolished by the EETC treatment.