Effects of electronic cigarette liquid on monolayer and 3D tissue-engineered models of human gingival mucosa

Zahab N Shaikh; Abdullah Alqahtani; Thafar Almela; Kirsty Franklin; Lobat Tayebi; Keyvan Moharamzadeh

doi:10.15171/japid.2019.010

Effects of electronic cigarette liquid on monolayer and 3D tissue-engineered models of human gingival mucosa

J Adv Periodontol Implant Dent. 2019 Dec 18;11(2):54-62. doi: 10.15171/japid.2019.010. eCollection 2019.

Authors

Zahab N Shaikh¹, Abdullah Alqahtani¹, Thafar Almela¹, Kirsty Franklin¹, Lobat Tayebi², Keyvan Moharamzadeh^{1

2}

Affiliations

¹ School of Clinical Dentistry, University of Sheffield, Claremont Crescent, Sheffield, S10 2TA, UK.
² Marquette University School of Dentistry, Milwaukee, WI 53233, USA.

Abstract

Background: There is limited data available on potential biological effects of E-cigarettes on human oral tissues. The aim of this study was to evaluate the effects of E-cigarette liquid on the proliferation of normal and cancerous monolayer and 3D models of human oral mucosa and oral wound healing after short-term and medium-term exposure.

Methods: Normal human oral fibroblasts (NOF), immortalized OKF6-TERET-2 human oral keratinocytes, and cancerous TR146 keratinocyte monolayer cultures and 3D tissue engineered oral mucosal models were exposed to different concentrations (0.1%, 1%, 5% and 10%) of E-cigarette liquid (12 mg/ml nicotine) for 1 hour daily for three days and for 7 days. Tissue viability was monitored using the PrestoBlue assay. Wounds were also produced in the middle surface of the monolayer systems vertically using a disposable cell scraper. The alterations in the cell morphology and wound healing were visualized using light microscopy and histological examination.

Results: Statistical analysis showed medium-term exposure of TR146 keratinocytes to 5% and 10% E-liquid concentrations significantly increased the viability of the cancer cells compared to the negative control. Short-term exposure of NOFs to 10% E-liquid significantly reduced the cell viability, whereas medium-term exposure to all E-liquid concentrations significantly reduced the NOF cells' viability. OKF6 cells exhibited significantly lower viability following short-term and mediumterm exposure to all E-cigarette concentrations compared to the negative control. 3D oral mucosal model containing normal oral fibroblasts and keratinocytes showed significant reduction in tissue viability after exposure to 10% E-liquid, whereas medium-term exposure resulted in significantly lower viability in 5% and 10% concentration groups compared to the negative control. There was a statistically significant difference in wound healing times of both NOF and OKF6 cells after exposure to 1%, 5% and 10% E-cigarette liquid.

Conclusion: Medium-term exposure to high concentrations of the E-cigarette liquid had cytotoxic effects on normal human oral fibroblasts and OKF6 keratinocytes, but a stimulatory cumulative effect on the growth of cancerous TR146 keratinocyte cells as assessed by the PrestoBlue assay and histological evaluation of 3D oral mucosal models. In addition, E-liquid exposure prolonged the wound healing of NOF and OKF6 oral mucosa cells.

Keywords: Electronic cigarette; cytotoxicity; fibroblast; keratinocyte; tissue engineering; wound healing.

Grants and funding

Funding: This research received no external funding.