Pre‐conditioning of gingival epithelial cells with sub‐apoptotic concentrations of curcumin prevents pro‐inflammatory cytokine release

Author:

Grant Melissa M.1ORCID,Scott Ann E.2,Matthews John B.1,Griffiths Helen R.3,Chapple Iain L. C.1

Affiliation:

1. Periodontal Research Group, School of Dentistry, Institute of Clinical Sciences and National Institute of Health Research (NIHR) Birmingham Biomedical Research Centre University of Birmingham and Birmingham Dental Hospital Birmingham UK

2. Unilever Oral Care Bebington, Wirral UK

3. Swansea University Swansea UK

Abstract

AbstractBackground and ObjectivePlaque‐induced gingival inflammation (gingivitis) is ubiquitous in humans. The epithelial barrier reacts to the presence of oral bacteria and induces inflammatory cascades. The objective of this study was to investigate the mechanism by which the small molecule micronutrient curcumin could decrease inflammatory response in vitro to oral bacterium heat‐killed Fusobacterium nucleatum as curcumin could be a useful compound for combatting gingivitis already consumed by humans.MethodsH400 oral epithelial cell line was pre‐conditioned with curcumin and the production of cytokines was measured by enzyme‐linked immunosorbent assay (ELISA) and translocation of transcription factors was used to monitor inflammatory responses. Haem oxygenase (HO‐1) expression and molecules that HO‐1 releases were evaluated for their potential to reduce the quantity of cytokine production. Immunofluorescence microscopy and Western blotting were used to evaluate changes in transcription factor and enzyme location.ResultsPre‐conditioning of H400 cells with a sub‐apoptotic concentration of curcumin (20 μM) attenuated secretion of Granulocyte‐Macrophage – Colony‐Stimulating Factor (GM‐CSF) and reduced NFkB nuclear translocation. This pre‐conditioning caused an increase in nuclear Nrf2; an initial drop (at 8 h) followed by an adaptive increase (at 24 h) in glutathione; and an increase in haem oxygenase (HO‐1) expression. Inhibition of HO‐1 by SnPPIX prevented the curcumin‐induced attenuation of GM‐CSF production. HO‐1 catalyses the breakdown of haem to carbon monoxide, free iron and biliverdin: the HO‐1/CO anti‐inflammatory pathway. Elevations in carbon monoxide, achieved using carbon monoxide releasing molecule‐2 (CORM2) treatment alone abrogated F. nucleatum‐induced cytokine production. Biliverdin is converted to bilirubin by biliverdin reductase (BVR). This pleiotropic protein was found to increase in cell membrane expression upon curcumin treatment.ConclusionCurcumin decreased inflammatory cytokine production induced by Fusobacterium nucleatum in H400 oral epithelial cells. The mechanism of action appears to be driven by the increase of haem oxygenase and the production of carbon monoxide.

Funder

Unilever

Publisher

Wiley

Subject

Periodontics

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