Strategies for the Covalent Anchoring of a BMP-2-Mimetic Peptide to PEEK Surface for Bone Tissue Engineering

Author:

Cassari Leonardo1ORCID,Zamuner Annj2ORCID,Messina Grazia Maria Lucia3ORCID,Marsotto Martina4ORCID,Chang Hao-chen5,Coward Trevor5ORCID,Battocchio Chiara4ORCID,Iucci Giovanna4ORCID,Marletta Giovanni3,Di Silvio Lucy5,Dettin Monica1ORCID

Affiliation:

1. Department of Industrial Engineering, University of Padova, Via Marzolo 9, 35131 Padova, Italy

2. Department of Civil, Environmental, and Architectural Engineering, University of Padova, Via Marzolo 9, 35131 Padova, Italy

3. Laboratory for Molecular Surface and Nanotechnology (LAMSUN), Department of Chemical Sciences, University of Catania and CSGI, Viale A. Doria, 6, 95125 Catania, Italy

4. Department of Science, Roma Tre University, Via della Vasca Navale 79, 00146 Roma, Italy

5. Faculty of Dentistry, Oral & Craniofacial Sciences, King’s College London, London SE1 9RT, UK

Abstract

Researchers in the field of tissue engineering are always searching for new scaffolds for bone repair. Polyetheretherketone (PEEK) is a chemically inert polymer that is insoluble in conventional solvents. PEEK’s great potential in tissue engineering applications arises from its ability to not induce adverse reactions when in contact with biological tissues and its mechanical properties, which are similar to those of human bone. These exceptional features are limited by the bio-inertness of PEEK, which causes poor osteogenesis on the implant surface. Here, we demonstrated that the covalent grafting of the sequence (48–69) mapped on the BMP-2 growth factor (GBMP1α) significantly enhances the mineralization and gene expression of human osteoblasts. Different chemical methods were employed for covalently grafting the peptide onto 3D-printed PEEK disks: (a) the reaction between PEEK carbonyls and amino-oxy groups inserted in the peptides’ N-terminal sites (oxime chemistry) and (b) the photoactivation of azido groups present in the peptides’ N-terminal sites, which produces nitrene radicals able to react with PEEK surface. The peptide-induced PEEK surface modification was assessed using X-ray photoelectron measurements, while the superficial properties of the functionalized material were analyzed by means of atomic force microscopy and force spectroscopy. Live and dead assays and SEM measurements showed greater cell cover on functionalized samples than the control, without any cytotoxicity induction. Moreover, functionalization improved the rate of cell proliferation and the amount of calcium deposits, as demonstrated by the AlamarBlue™ and alizarin red results, respectively. The effects of GBMP1α on h-osteoblast gene expression were assayed using quantitative real-time polymerase chain reaction.

Publisher

MDPI AG

Subject

General Materials Science

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