Efficacy of bioactive nanoparticles on tissue-endotoxin induced suppression of stem cell viability, migration and differentiation

H Kukreti; F-C Li; K Singh; R Sodhi; A Kishen

doi:10.1111/iej.13283

Efficacy of bioactive nanoparticles on tissue-endotoxin induced suppression of stem cell viability, migration and differentiation

Int Endod J. 2020 Jun;53(6):859-870. doi: 10.1111/iej.13283. Epub 2020 Mar 13.

Authors

H Kukreti¹, F-C Li¹, K Singh¹, R Sodhi², A Kishen¹

Affiliations

¹ Faculty of Dentistry, Dental Research Institute, University of Toronto, Toronto, Ontario, Canada.
² Ontario Centre for the Characterization of Advanced Materials (OCCAM), Department of Chemical Engineering and Applied Chemistry, University of Toronto, Toronto, Ontario, Canada.

PMID: 32068891
DOI: 10.1111/iej.13283

Abstract

Aim: To characterize a lipopolysaccharide (LPS)-treated dentine tissue model (LPS dentine) to analyse the efficacy of polycationic chitosan nanoparticles (CSnp) and/or dexamethasone conjugate chitosan nanoparticles (Dex-CSnp) on the viability/differentiation potential of stem cells from apical papilla (SCAP) when exposed to LPS dentine. A further aim was to understand the effect of macrophage-dependent inflammation on SCAP migration in the presence of LPS dentine.

Methodology: A total of 88 dentine slabs were used. TOF-SIMS analysis was performed amongst the LPS-treated and untreated dentine groups (n = 2/group). The study was conducted using four dentine groups: no treatment (control); LPS treatment only; LPS treatment followed by CSnp conditioning; and LPS treatment followed by Dex-CSnp conditioning groups. SCAP adherence, viability, differentiation and biomineralization potential on dentine from different groups were studied using fluorescent and scanning electron microscopy. Inflammation by macrophages in response to LPS dentine was quantified, and effect on SCAP migration was analysed. Statistical analysis was performed using Student's t-test with a significance level of P < 0.05.

Result: TOF-SIMS analysis confirmed LPS contamination. LPS dentine affected SCAP viability but not adherence to dentine (P < 0.001). Conditioning of LPS dentine with either nanoparticles improved SCAP viability (P < 0.01) and rescued other LPS related adverse effects on SCAPs, such as F-actin disruption, decrease in differentiation/biomineralization potential. IL-6 produced by macrophages in response to LPS-treated dentine impeded SCAP migration (P < 0.001), diminished on CSnp and Dex-CSnp conditioning groups (P < 0.01).

Conclusion: This study developed an LPS-dentine model and highlighted the ability of CSnp and Dex-CSnp to promote stem cell viability, migration, differentiation potential and reduce inflammation, providing an environment conducive for tissue regeneration/repair.

Keywords: SCAPs; chitosan nanoparticles; endotoxin.

MeSH terms

Cell Differentiation
Cell Survival
Chitosan*
Dental Papilla
Humans
Nanoparticles*
Stem Cells

Substances

Chitosan

Grants and funding

206760/University of Toronto