Abstract
A close causal relationship has been suggested to exist between cancer and periodontitis. We hypothesized that the immune surveillance system is impaired in patients with periodontitis, which contributes to cancer development and growth. Therefore, the present study investigated the relationship between immune surveillance mechanisms and periodontitis in cancer patients. The presence or absence of periodontitis was assessed and the peripheral blood (PB) concentrations of IL-6, immunosuppressive cytokines (VEGF, TGF-β1, and CCL22) and proportion of T regulatory cells (Treg, CD3 + CD4 + CD25 + Foxp3 +) were measured. Subjects were classified into the following four groups: non-cancer patients without periodontitis (C − P −), non-cancer patients with periodontitis (C − P +), cancer patients without periodontitis (C + P −), and cancer patients with periodontitis (C + P +). The results of a multivariate analysis showed that the PB concentration of IL-6 was significantly higher in C + than in C- and higher in C + P + than in C + P −. The PB proportion of Treg was significantly higher in C + P + than in C + P −, C − P + , and C − P −. The results of this study suggested that the presence of periodontitis and cancer synergistically increased Treg in PB, which may be one of the underlying causes of immunosuppression and immune evasion in cancer. It was also suggested that the presence of periodontal disease and/or cancer also increases IL-6 in PB, which would be associated with cancer progression. These results suggest the possibility that the presence of periodontitis might synergistically contribute to cancer progression.
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Introduction
Cancer immunity has been attracting increasing attention in recent years. In the process of cancer development and proliferation, cancer evades immune surveillance via a number of mechanisms. Two mechanisms have been confirmed: immunosuppression triggered by genetic aberrations in cancer cells and that by antitumor T cells that have already been induced1,2. In the former, genetic abnormalities in cancer cells induce interleukin-6 (IL-6) and immunosuppressive cytokines, such as transforming growth factor-β (TGF-β), interleukin-10 (IL-10), vascular endothelial growth factor (VEGF), and macrophage-derived chemokine (CCL22), as well as immunosuppressive cells [regulatory T cells (Treg) and bone marrow-derived immunosuppressive cells], which suppress the function of dendritic cells and antitumor T cells3.
The relationship between periodontal disease and cancer has been the focus of research based on findings showing that the risk of cancer development and cancer mortality are higher in patients with periodontal disease4,5,6,7,8,9,10,11,12. We also reported that the prevalence of severe periodontitis was higher in cancer patients13. However, the mechanisms contributing to this relationship remain unclear. A recent study showed that the number of Treg cells in peripheral blood (PB) was significantly higher in patients with periodontal disease than in those without periodontal disease14. Periodontitis, an inflammatory disease, is caused by oral microbiota, including P. gingivalis, Treponema denticola, and Tannerella forsythia15. Gingipain proteases produced by P. gingivalis affect the integrity of the cytokines IL-6 which are produced in response to the infection16.
Periodontitis develops and progresses as a result of an interaction between the immune system of the host and periodontal pathogens. Cytokines and immune cells play a crucial role in the modulation of host–pathogen homeostasis17. Treg are a key immunoregulatory element that has an anergic phenotype and plays an important role in the suppression of exacerbated immune responses, thereby maintaining homeostasis, which also preserves physiological/functional tissue homeostasis14,18. Present periodontitis affected systemic disease such as diabetes, atherosclerosis. Several previous studies indicated that higher prevalence of periodontitis in diabetic patients, and IL-6 might mediate periodontitis in diabetes19,20. And others studies showed that A. actinomycetemcomitans, P. gingivalis, T. forsythia, T. denticola, and F. nucleatumare related to higher risk of atherosclerosis, and some cardiovascular diseases are related to chronic inflammation21. Therefore, the presence of chronic inflammation, such as periodontitis, in the body may reduce systemic immune surveillance functions (e.g., increases in Treg), which may, in turn, promote the development and progression of cancer.
Based on these findings, we hypothesized that the immune surveillance system is impaired in patients with periodontitis, which contributes to cancer development and growth. Therefore, the present study investigated the relationship between immune surveillance mechanisms and periodontal disease in cancer patients.
Materials and methods
The study protocol was approved by the Ethics Committee of Shinshu University School of Medicine (Approval number #4144). The present study was performed in accordance with the Declaration of Helsinki (2013 Fortaleza revision) and Ethical Guidelines for Medical Research for Humans.
Patients
Subjects were recruited for the present study from patients who attended the Oral Management Center of Shinshu University Hospital and the Oral Disease Center of Aizawa Hospital between November 2018 and March 2020. Inclusion and exclusion criteria are summarized in Table 1. Data that may influence immunosuppression, cancer, or periodontitis (age, sex, smoking status (the Brinkman index), diabetes mellitus (DM), and number of teeth) were retrieved from patient medical records.
Assessment of periodontitis
We conducted an oral examination and periodontal disease assessment according to the Standard Adult Dental Examination Program/Health Guidance Manual (Japan Dental Association) and Periodontal disease screening program 2015 (Ministry of Health, Labour and Welfare, https://www.mhlw.go.jp/file/06-Seisakujouhou-10900000-Kenkoukyoku/manual2015.pdf) including a radiological examination using dental panoramic radiographs. Patients a probing depth < 3 mm, no bleeding on probing, and no radiographic evidence of horizontal alveolar bone loss were classified did not have periodontitis, while those with the opposite findings had periodontitis. Diagnosis of periodontal disease by clinical and imaging examination was performed by experienced dentists with prior training.
PB sample collection and component analysis
PB was collected from the antecubital vein into EDTA-coated vacutainer tubes and thrombin-coated vacutainer tubes. Peripheral blood mononuclear cells (PBMC) obtained from the former were used for a flow cytometry (FCM) analysis and serum from the latter to analysis IL-6, VEGF, TGF-β1, and CCL22 concentrations measured by SRL Ltd. (Tokyo, Japan) and LSI Medience Corporation Ltd. (Tokyo, Japan).
FCM analysis
Foxp3 is a specific marker of Treg. PBMC were separated from collected blood samples and Treg were detected by the expression of CD25 and Foxp3. We used the following fluorochrome-conjugated antibodies to stain the cell surface antigens: PerCp/Cy5.5 anti-human CD3, Brilliant Violet 421 anti-human CD4, APC anti-human CD25 (BioLegend, San Diego, CA, USA), and Ghost Rad780 Viability dye (Tonbo Bioscience, San Diego, CA, USA). We permeabilized cells using a Human Foxp3 buffer set kit (BD Bioscience, San Diego, CA USA), and stained Foxp3 using PE anti-human Foxp3 (BioLegend, San Diego, CA, USA). FCM was performed using BD FACS CantoII(Ver1.1, Diva6.1, BD Bioscience, San Diego, CA USA) and BD FACSDiva9, FlowJo (BD Bioscience, San Diego, CA USA) was used for data analysis. The gating strategy for the isolation of Treg involved the following steps: (1) isolation of live cells, (2) gating to isolate CD3- and CD4-positive cells, and (3) isolation of CD25- and Foxp3-positive cells (Supplementary Fig. 1).
Statistical analysis
Statistical analyses, including Pearson’s test, the Wilcoxon test, Pearson’s correlation coefficient, Spearman’s correlation coefficient by rank, Tukey’s HSD test, the Steel–Dwass test, and a multivariate regression analysis, were performed using PC software (JMP v13.2, SAS Inc., NC, USA). All p-values < 0.5 were considered to indicate statistical significance.
Results
Thirty cancer and 31 non-cancer patients agreed with informed consent to participate in the present study. Tumor sites in cancer patients were the head and neck (12 patients), lungs (5), colon (4), pancreas (3), breast (2), esophagus (2), duodenum (1), and bile duct (1). Among the 61 patients enrolled in the present study, 42 were diagnosed with periodontitis. Patients were classified into the following four groups: non-cancer patients without periodontitis (C − P −, 14 patients), non-cancer patients with periodontitis (C − P + , 17), cancer patients without periodontitis (C + P −, 5), and cancer patients with periodontitis (C + P + , 25). The characteristics of each group are shown in Table 2. Significant differences were observed in age, the Brinkman index, and the number of teeth among the groups. Mean age was lower in the C − P − group than in the other groups (p < 0.01). The Brinkman index was higher in the C + P + group than in the C − groups (p < 0.05). The number of teeth was significantly lower in the C + P + group than in the C − P − group (p < 0.01).
The results of a univariate analysis of the relationship between the levels of IL-6, immunosuppressive molecules or proportion of Treg and influencing factors (sex, age, the Brinkman index, DM, number of teeth, presence/absence of cancer, and periodontitis) are summarized in Table 3. No correlations were observed between TGF-β1, VEGF, or CCL22 concentrations and sex, the presence/absence of DM, age, the Brinkman index, or the number of teeth. Furthermore, no correlations were noted between TGF-β1, VEGF, or CCL22 concentrations and the presence/absence of cancer and/or periodontitis. On the other hand, correlations were detected between the concentration of IL-6 and either the presence/absence of DM or cancer/periodontitis. IL-6 concentrations were significantly higher in DM patients than in non-DM patients (median 4.3 vs. 1.5 pg/mL, P < 0.01), and were lower in C − P − patients than in the three other groups (median 0.7 vs. 2.2, 2.6, and 2.8 pg/mL, P < 0.05; Fig. 1A). In addition, a correlation was observed between the proportion of Treg and cancer/periodontitis. The proportion of Treg was significantly higher in C + P + patients than in C − P + patients (median 3.78 vs. 2.11%, p < 0.05; Figs. 1B and 2). And the proportion of Treg in PB was slightly higher in cancer patients than in non-cancer patients [median (IQR); 3.515% (2.1925–4.9875) vs. 2.56% (1.83–3.6975), p = 0.052]. However, no significant differences were observed in PB Treg between patients with and without periodontitis [median (IQR); 3.105% (2.0875–4.7625) vs. 3.16% (2.17–3.9775), p = 0.826].
The result of multivariate analysis is shown in Table 4. The relationships between either IL-6 concentrations or the proportion of Treg and influencing factors were analyzed. Regarding IL-6, the presence of cancer and the presence of periodontitis in cancer patients had a significant impact on the PB concentration of IL-6 (C − vs. C + , estimate − 7.534, p < 0.05 and C + P + vs C + P −, estimate 14.903, p < 0.01). Concerning Treg, the presence of both cancer and periodontitis had a significant impact on the PB proportion of Treg (C − and C + P − vs. C + P + , estimate − 0.774, p < 0.01). Age also had a significant impact on the proportion of Treg (estimate − 0.033, p < 0.05). These results of the multivariate analysis adjusted for confounding factors showed that the presence of cancer and/or periodontitis was associated with a higher PB concentration of IL-6 and proportion of Treg.
Discussion
The present study is the first to examine the relationship between periodontitis and cancer from the aspect of immune surveillance mechanisms. We herein assessed the proportion of immunosuppressive cells and levels of IL-6 and immunosuppressive cytokines in the PB of patients with periodontal disease and/or cancer. Patients were classified into the four groups (C − P −, C − P + , C + P −, and C + P +) for comparison.
In the present study, PB levels of IL-6 and the proportion of Treg correlated with the presence and absence of cancer and/or periodontitis in both the univariate and multivariate analyses. Age and the smoking status significantly differed among the four groups compared in the present study. This was expected because the incidence of cancer and periodontal disease increases with age. Since age and the smoking status are considered to affect the immune status of the host22,23, adjustments for these confounding factors were warranted. Differences in the number of remaining teeth were also observed, but were naturally expected because periodontal disease is the most common reason for tooth loss in middle-aged and older individuals. Differences in the concentrations of pro-inflammatory cytokines according to the number of teeth affected by periodontal disease also need to be considered and their influence warrants further study. The results of the multivariate analysis adjusted for confounding factors showed that the presence of cancer and/or periodontitis was associated with a higher PB concentration of IL-6 and proportion of Treg, confirming the influence of the presence of cancer and periodontitis on the immune surveillance system of the host.
In this study the number of cancer patients without periodontitis (5 patients in C + P −) was smaller than in the other groups. Cancer and periodontal disease are both common in middle-aged and older individuals, and the prevalence of periodontal disease is higher in cancer patients13. We considered this imbalance in the number of patients to be unavoidable and proceeded with analyses. However, in the results of this study, the C + P + group had a significantly higher percentage of Tregs than the other three groups. This result suggests the existence of a synergistic effect between periodontal disease and cancer.
The concentration of IL-6 was significantly higher in patients with cancer and/or periodontitis than in those with neither cancer nor periodontitis. Previous studies suggested that IL-6 was associated with periodontitis. Salivary concentrations of IL-6 were shown to be higher in chronic periodontitis patients than in healthy controls24,25. Pro-inflammatory and anti-inflammatory cytokines have been detected in periodontal lesions, gingival crevice fluid, and gingival cells26. Furthermore, high expression levels of proinflammatory cytokines, including IL-6, were found in periodontitis and triggered osteoclast activity, which caused bone resorption27. IL-6 is also one of the major cytokines in cancer and plays a key role in cancer progression, metastasis, and therapeutic resistance28. It exerts direct stimulatory effects on many cancer cells through several signal pathways29,30. The present results revealed that IL-6 concentrations were increased in PB, but not in the cancer/periodontitis microenvironment. Higher levels of cytokines, including IL-6, in PB have been reported in patients with periodontitis31 and cancer32, which is consistent with the present results. The presence of local cancer or periodontal disease induced a higher PB level of IL-6, which may influence the general health of patients or may be associated with the development/progression of other diseases. We speculated that IL-6 from periodontitis may play a role in the development/progression of cancer. Cancer may be involved in the development/progression of periodontal disease and vice versa. IL-6 derived from gingival fibroblast induced VEGF through infiltrated macrophages in periodontitis site33. And TGF-β is also induced periodontitis site and play a role in wound healing and immunosuppression action34. In cancer site, overproduction of TGF-β induce immunosuppression in tumor and in lymph nodes, through Treg and myeloid-derived suppressor cells induction35. And VEGF has a dual function in supporting tumor progression, by inducing vessel formation and by acting as an immunosuppressive factor36. However, in this study, concentration of VEGF and TGF-β1 in PB was not significant differences between each group. We need to further study correlation between cancer and periodontitis regarding immunosuppressive cytokines.
The proportion of Treg in PB was significantly higher in patients with both cancer and periodontitis than in those without cancer or in cancer patients without periodontitis. This result suggests that the presence of periodontitis in cancer patients resulted in an additional increase in the proportion of Treg in PB. To the best of our knowledge, this is the first study to report a synergistic relationship between periodontitis and cancer in Treg-mediated immunosuppression.
CD4+CD25+Treg expressing the transcriptional factor Foxp3 are highly immunosuppressive and play central roles in the maintenance of self-tolerance and immune homeostasis37,38. Treg may suppress anticancer immunity, thereby hindering the protective immunosurveillance of neoplasia and hampering effective antitumor immune responses in tumor-bearing hosts, ultimately promoting tumor development and progression39. Elevated levels of Treg in the local microenvironment of cancer and a strong relationship between Treg and a poor prognosis in various types of cancer have been reported40. Furthermore, circulating Treg cells were shown to be elevated in several cancers and correlated with a poor prognosis41,42. In the present study, the proportion of Treg in PB was slightly higher in cancer patients than in non-cancer patients [median (IQR); 3.515% (2.1925–4.9875) vs. 2.56% (1.83–3.6975), p = 0.052].
Higher levels of Treg have been reported in the gingival tissues and PB of patients with chronic periodontitis14,43,44. Treg play a critical role in immunological tolerance and the suppression of inflammatory responses in the pathogenesis of periodontitis. In the present study, no significant differences were observed in PB Treg between patients with and without periodontitis [median (IQR); 3.105% (2.0875–4.7625) vs. 3.16% (2.17–3.9775), p = 0.826]. However, as noted above, a significant difference was observed between cancer patients with and without periodontitis. The presence of cancer and periodontal disease appears to synergistically increase Treg in PB. Previous studies reported that chronic and autoimmune diseases, such as rheumatoid arthritis (RA) and tuberculosis, had higher levels of Treg in the systemic circulation45,46,47. Patients with RA are at an increased risk of malignancies than the general population48. Periodontitis is a chronic inflammatory disease with compromised immunomodulatory mechanisms (immune tolerance). The systemic level of Treg is elevated with chronic or autoimmune disease, which may be one of the underlying causes of immunosuppression and immune evasion by cancer cells. These findings suggest that the presence of periodontitis contributes to immune evasion in cancer. In addition, the proportion of Treg was significantly lower with advancing age, which may reflect a decrease in the induction of Treg because of immune tolerance with aging49.
Previous studies demonstrated the importance of CCL22 in the migration of Treg50,51. In the present study, no significant differences were observed in the PB concentration of CCL22 in both cancer and/or periodontitis patients. Wertel et al. examined the PB, peritoneal fluid (PF), and tissue levels of CCL22 and Treg in patients with ovarian cancer, and reported that the percentage of Treg infiltrating tumors was significantly higher than in PF and PB, while no significant differences were noted in PB CCL22 concentrations between ovarian cancer patients and non-cancer patients52. CCL22 may be produced locally by tumor cells and myeloid dendritic cell2, and was also increased at periodontal inflammation sites53,54. These findings indicate that an increase of CCL22 in PB was not observed in patients with cancer or periodontitis because CCL22 increased locally and induced the migration of Treg.
In this study, we classified patients with a probing depth > 3 mm, bleeding on probing, and radiographic evidence of horizontal alveolar bone loss were classified with periodontitis. Our classification was different from the new EFP/AAP classification, and our classification might be insatisfaction. However, our result showed correlation presence destruction of periodontal tissue and cancer through Treg and IL-6 involved. And it was remained unclear, the duration of differences between periodontitis and cancer development, and immune response of the immune system concerned. Our result suggested that underlying periodontitis, no relevant the duration the time of development, might contribute cancer invasion through immune imbalance. Current study is the first report of correlation presence of periodontitis and cancer, but we need to further study to make clear presence of periodontitis contribution to cancer invasion.
In conclusion, we showed that the presence of periodontitis and cancer synergistically increased Treg in PB, which may be one of the underlying causes of immunosuppression and immune evasion in cancer. The presence of periodontal disease and/or cancer also increases IL-6 in PB, which would be associated with cancer progression. These results suggest the possibility that the presence of periodontitis might synergistically contribute to cancer progression.
Data availability
The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request.
References
Beatty, G. L. & Gladney, W. L. Immune escape mechanisms as a guide for cancer immunotherapy. Clin. Cancer Res. 21(4), 687–692 (2015).
Nishikawa, H. & Sakaguchi, S. Regulatory T cells in tumor immunity. Int. J Cancer. 127(4), 759–767 (2010).
Yaguchi, T. & Kawakami, Y. Cancer-induced heterogeneous immunosuppressive tumor microenvironments and their personalized modulation. Int. Immunol. 28(8), 393–399 (2016).
Michaud, D. S., Liu, Y., Meyer, M., Giovannucci, E. & Joshipura, K. Periodontal disease, tooth loss, and cancer risk in male health professionals: A prospective cohort study. Lancet Oncol. 9(6), 550–558 (2008).
Corbella, S. et al. Is periodontitis a risk indicator for cancer? A meta-analysis. PLoS One 13(4), 0195683 (2018).
Michaud, D. S. et al. Periodontal disease assessed using clinical dental measurements and cancer risk in the ARIC study. J. Natl Cancer Inst. 110(8), 843–854 (2018).
Gasparoni, L. M., Alves, F. A., Holzhausen, M., Pannuti, C. M. & Serpa, M. S. Periodontitis as a risk factor for head and neck cancer. Med. Oral. Patol. Oral. Cir. Bucal. 26(4), e430-436 (2021).
Wang, J. et al. Relationship between periodontal disease and lung cancer: A systematic review and meta-analysis. J. Periodontal. Res. 55(5), 581–593 (2020).
Maisonneuve, P., Amar, S. & Lowenfels, A. B. Periodontal disease, edentulism, and pancreatic cancer: A meta-analysis. Ann. Oncol. 28(5), 985–995 (2017).
Xuan, K., Jha, A. R., Zhao, T., Uy, J. P. & Sun, C. Is periodontal disease associated with increased risk of colorectal cancer? A meta-analysis. Int. J. Dent. Hyg. 19(1), 50–61 (2021).
Heikkilä, P., But, A., Sorsa, T. & Haukka, J. Periodontitis and cancer mortality: Register-based cohort study of 68,273 adults in 10-year follow-up. Int. J. Cancer. 142(11), 2244–2253 (2018).
Ahn, J., Segers, S. & Hayes, R. B. Periodontal disease, Porphyromonas gingivalis serum antibody levels and orodigestive cancer mortality. Carcinogenesis 33(5), 1055–1058 (2012).
Sakai, H. et al. A retrospective analysis of the prevalence of dental diseases in patients with digestive system cancers. Medicine (Baltimore) 98(13), 14771. https://doi.org/10.1097/MD.0000000000014771 (2019).
Sabarish, R., Bao, S. R. & Lavu, V. Natural T regulatory cell (n Treg) in the peripheral blood of healthy subjects and subjects with chronic periodontitis - A pilot study. J. Clin. Diag. Res. 10(3), ZC36-39 (2016).
Socransky, S. S. et al. Use of checkerboard DNA-DNA hybridization to study complex microbial ecosystems. Oral. Microbiol. Immunol. 19(6), 352–362 (2004).
Banbula, A. et al. Rapid and efficient inactivation of IL-6 gingipains, lysine- and arginine-specific proteinases from Porphyromonas gingivalis. Biochem. Biophys. Res. Commun. 261(3), 598–602 (1999).
Pan, W., Wang, Q. & Chen, Q. The cytokine network involved in the host immune response to periodontitis. Int. J. Oral Sci. https://doi.org/10.1038/s41368-019-0064-z (2019).
Alvarez, C. et al. Regulatory T Lymphocytes in periodontitis: A translational view. Mediators Inflamm. https://doi.org/10.1155/2018/7806912 (2018).
Khader, Y. S., Dauod, A. S., El-Qaderi, S. S., Alkafajei, A. & Batayha, W. Q. Periodontal status of diabetics compared with nondiabetics: A meta-analysis. J. Diabetes Complicat. 20(1), 59–68 (2006).
Taylor, J. J., Preshaw, P. M. & Lalla, E. A review of the evidence for pathogenic mechanisms that may link periodontitis and diabetes. J. Clin. Periodontol. 40, S113–S134 (2013).
Bale, B. F., Doneen, A. L. & Vigerust, D. J. High-risk periodontal pathogens contribute to the pathogenesis of atherosclerosis. Postgrad. Med. J. 93(1098), 215–220 (2017).
Pawelec, G. Age and immunity: What is “immunosenescence”?. Exp Gerontol. 105, 4–9 (2018).
Mehta, H., Nazzal, K. & Sadikot, R. T. Cigarette smoking and innate immunity. Inflamm. Res. 57(11), 497–503 (2008).
Keles Yucel, Z. P., Keles, G. C., Avci, B. & Cetinkaya, B. O. Nonsurgical periodontal therapy reduces salivary and gingival crevicular fluid YKL-40 and IL-6 levels in chronic periodontitis. Oral Health Prev. Dent. 18(1), 815–822 (2020).
Batool, H. et al. Salivary levels of IL-6 and IL-17 could be an indicator of disease severity in patients with calculus associated chronic periodontitis. Biomed. Res. Int. https://doi.org/10.1155/2018/8531961 (2018).
Pan, W., Wang, Q. & Chen, Q. The cytokine network involved in the host immune response to periodontitis. Int. J. Oral Sci. 11(3), 30. https://doi.org/10.1038/s41368-019-0064-z (2019).
Ramadan, D. E., Hariyani, N., Indrawati, R., Ridwan, R. D. & Diyatri, I. Cytokines and chemokines in periodontitis. Eur. J. Dent. 3, 483–495 (2020).
Kumari, N., Dwarakanath, B. S., Das, A. & Bhatt, A. N. Role of interleukin-6 in cancer progression and therapeutic resistance. Tumour. Biol. 37(9), 11553–11572 (2016).
Guo, Y., Xu, F., Lu, T., Duan, Z. & Zhang, Z. Interleukin-6 signaling pathway in targeted therapy for cancer. Cancer Treat Rev. 38(7), 904–910 (2012).
Ara, T. & Declerck, Y. A. Interleukin-6 in bone metastasis and cancer progression. Eur. J. Cancer. 46(7), 1223–1231 (2010).
Gonçalves, T. O. et al. Release of cytokines by stimulated peripheral blood mononuclear cells in chronic periodontitis. Arch. Oral Biol. 55(12), 975–980 (2010).
Wang, L. et al. IL6 signaling in peripheral blood T cells predicts clinical outcome in breast cancer. Cancer Res. 77(5), 1119–1126 (2017).
Naruishi, K. & Nagata, T. Biological effects of interleukin-6 on gingival fibroblasts: Cytokine regulation in periodontitis. J. Cell Physiol. 233(9), 6393–6400 (2018).
Jakhu, H., Gill, G. & Singh, A. Role of integrins in wound repair and its periodontal implications. J. Oral Biol. Craniofac. Res. 8(2), 122–125 (2018).
Nakamura, S. et al. TGF-β1 in tumor microenvironments induces immunosuppression in the tumors and sentinel lymph nodes and promotes tumor progression. J. Immunother. 37(2), 63–72 (2014).
Li, Y. L., Zhao, H. & Ren, X. B. Relationship of VEGF/VEGFR with immune and cancer cells: Staggering or forward?. Cancer Biol. Med. 13(2), 206–214 (2016).
Li, Z., Li, D., Tsun, A. & Li, B. FOXP3+ regulatory T cells and their functional regulation. Cell Mol. Immunol. 12(5), 558–565 (2015).
Sakaguchi, S., Yamaguchi, T., Nomura, T. & Ono, M. Regulatory T cells and immune tolerance. Cell 133(5), 775–787 (2008).
Togashi, Y., Shitara, K. & Nishikawa, H. Regulatory T cells in cancer immunosuppression - Implications for anticancer therapy. Nat. Rev. Clin. Oncol. 16(6), 356–371 (2019).
Takeuchi, Y. & Nishikawa, H. Roles of regulatory T cells in cancer immunity. Int. Immunol. 28(8), 401–409 (2016).
Sawan, S. et al. Circulating regulatory T cells in endometrial cancer: A role for age and menopausal status. Immunol. Invest. 40(1), 62–75 (2011).
Kotsakis, A. et al. Prognostic value of circulating regulatory T cell subsets in untreated non-small cell lung cancer patients. Sci. Rep. 6, 39247 (2016).
Cardoso, C. R. et al. Characterization of CD4+CD25+ natural regulatory T cells in the inflammatory infiltrate of human chronic periodontitis. J. Leukoc. Biol. 84(1), 311–318 (2008).
Nakajima, T. et al. Regulatory T-cells infiltrate periodontal disease tissues. J. Dent. Res. 84(7), 639–643 (2005).
Kao, J. K., Hsue, Y. T. & Lin, C. Y. Role of new population of peripheral CD11c+CD8+ T cells and CD4+CD25+ regulatory T cells during acute and remission stages in rheumatoid arthritis patients. J. Microbiol. Immunol. Infect. 40(5), 419–427 (2007).
Cao, D. et al. Isolation and functional characterization of regulatory CD25brightCD4+ T cells from the target organ of patients with rheumatoid arthritis. Eur. J. Immunol. 33(1), 215–223 (2001).
Guyot-Revol, V., Innes, J. A., Hackforth, S., Hinks, T. & Lalvani, A. Regulatory T cells are expanded in blood and disease sites in patients with tuberculosis. Am. J. Respir. Crit. Care Med. 173(7), 803–810 (2006).
Simon, T. A., Thompson, A., Gandhi, K. K., Hochberg, M. C. & Suissa, S. Incidence of malignancy in adult patients with rheumatoid arthritis: A meta-analysis. Arthritis. Res. Ther. 17(1), 212 (2015).
Carpentier, M. et al. Extrathymic induction of Foxp3+ regulatory T cells declines with age in a T-cell intrinsic manner. Eur. J. Immunol. 43(10), 2598–2604 (2013).
Iellem, A. et al. Unique chemotactic response profile and specific expression of chemokine receptors CCR4 and CCR8 by CD4+ CD25+ regulatory T cells. J. Exp. Med. 194(6), 847–853 (2001).
Gobert, M. et al. Regulatory T cells recruited through CCL22/ CCR4 are selectively activated in lymphoid infiltrates surrounding primary breast tumors and lead to an adverse clinical outcome. Cancer Res. 69(5), 2000–2009 (2009).
Wertel, I. et al. Macrophage-derived chemokine CCL22 and regulatory T cells in ovarian cancer patients. Tumour Biol. 36(6), 4811–4817 (2015).
Araujo-Pires, A. C. et al. IL-4/CCL22/CCR4 axis controls regulatory T-cell migration that suppresses inflammatory bone loss in murine experimental periodontitis. J. Bone Miner. Res. 30(3), 412–422 (2015).
Cardoso, C. R. et al. Characterization of CD4+CD25+ natural regulatory T cells in the inflammatory infiltrate of human chronic periodontitis. J. Leukoc. Biol. 84(1), 311–318 (2008).
Acknowledgements
We thank Nobuhiko Yoshimura in Oral Disease Center of Aizawa Hospital recruited subjects and collected peripheral blood sample.
Funding
This study was supported by JPS KAKENHI Grant Number JP21K16943.
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R.K. and H.S. wrote manuscript, performed the experiments, and analyzed data. H.Y., K.A., M.K., Y.H., and S.N. performed the experiments, and analyzed data. S.Y., H.S. and H.S. designed the experiments and analyzed data. H.K. wrote manuscript, designed the experiments and analyzed data.
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Kajihara, R., Sakai, H., Han, Y. et al. Presence of periodontitis may synergistically contribute to cancer progression via Treg and IL-6. Sci Rep 12, 11584 (2022). https://doi.org/10.1038/s41598-022-15690-w
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DOI: https://doi.org/10.1038/s41598-022-15690-w
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