Abstract
In this study we synthesized gelatin-based, tissue-engineering, interpenetrating network (IPN) scaffolds immobilized with fibronectin (FN)-derived peptides to assess monocyte–biomaterial interaction. Human promonocytic U937 cells were seeded onto peptide-grafted IPN or tissue-culture polystyrene plate (TCPS) pre-adsorbed with FN or FN-derived peptides. The presence of RGD influenced U937 density on IPN. Interleukin-1 beta (IL-1β) messenger ribonucleic acid (mRNA) expression in adherent U937 on treated TCPS was slightly upregulated at 4 h. Tumor necrosis factor alpha (TNF-α) and IL-1β mRNA expression in adherent U937 on all IPNs was generally downregulated at 4 h. This downregulation of IL-1β mRNA apparently varied in IPNs grafted with different ligand and was still present at 24 h. TNF-α and IL-1β proteins released from U937 on treated TCPS were comparable with the control at 24 h, but TNF-α and IL-1β protein expression in U937 on IPNs was lower at 24 h than on the TCPS control. The results indicate that the tissue-engineering substrate and the bioactive peptides modulate the initial U937 adhesion and the subsequent inflammatory cytokine gene and protein expression.
Get full access to this article
View all access options for this article.