CpG single-site methylation regulates tlr2 expression in proinflammatory PBMCs from apical periodontitis individuals
Author
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Bordagaray San Martín, María José
Author
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Fernández, Alejandra
Author
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Astorga, Jessica
Author
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Garrido Flores, Carlos Mauricio
Author
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Hernández Ríos, Patricia
Author
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Chaparro, Alejandra
Author
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Lira, María Jesús
Author
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Gebicke Haerter, Peter
Author
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Hernández Ríos, Emma
Admission date
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2022-06-30T21:09:38Z
Available date
dc.date.available
2022-06-30T21:09:38Z
Publication date
dc.date.issued
2022
Cita de ítem
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Frontiers in Immunology March 2022 Volume 13 Article 861665
es_ES
Identifier
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10.3389/fimmu.2022.861665
Identifier
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https://repositorio.uchile.cl/handle/2250/186377
Abstract
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IntroductionApical periodontitis (AP) is a common oral disease caused by the inflammatory destruction of the periapical tissues due to the infection of the root canal system of the tooth. It also contributes to systemic bacterial translocation, where peripheric mononuclear blood cells (PBMCs) can act as carriers. Toll-like receptor (TLR) 2 mediates the response to infection and activates inflammatory responses. DNA methylation can be induced by bacteria and contributes to the modulation of this response. Despite the evidence that supports the participation of PBMCs in immune-inflammatory disorders, the inflammatory profile and epigenetic regulatory mechanisms of PBMCs in AP individuals are unknown. AimTo determine TLR2 gene methylation and inflammatory profiles of PBMCs in AP. MethodsCross-sectional exploratory study. Otherwise, healthy individuals with AP (n=27) and controls (n=30) were included. PMBCs were isolated by a Ficoll gradient, cultured for 24 hours, and both RNA and DNA were extracted. DNA was bisulfite-treated, and specific sites at the promoter region of the TLR2 gene were amplified by qPCR using validated primers. To verify its amplification, agarose gels were performed. Then, the PCR product was sequenced. mRNA expression of TLR2 was determined by qPCR. The soluble levels of 105 inflammatory mediators were first explored with Proteome Profiler Human Cytokine Array Kit. Consequently, tumor necrosis factor (TNF)-alpha, interleukin (IL)-6, IL-10, IL-6R alpha, IL-1 beta, and IL-12p70 levels were measured by Multiplex assay. ResultsPBMCs from individuals with AP demonstrated a proinflammatory profile showing higher soluble levels of TNF-alpha, IL-6, and IL-1 beta compared to controls (p<0.05). Higher TLR2 expression and higher global methylation pattern of the promoter region of the gene were found in AP compared to controls (p<0.05). The CpGs single-sites at positions -166 and -146 were completely methylated, while the site -102 was totally unmethylated, independently of the presence of AP. DNA methylation of CpG single-sites in positions -77 and +24 was positively associated with TLR2 expression. ConclusionsPBMCs from AP subjects show a hyperinflammatory phenotype and TLR2 upregulation in association with single CpG-sites' methylation from the TLR2 gene promoter, thereby contributing to a sustained systemic inflammatory load in individuals with periapical endodontic diseases.
es_ES
Lenguage
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en
es_ES
Publisher
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Frontiers Media
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Type of license
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Attribution-NonCommercial-NoDerivs 3.0 United States