Bone Defect Repair Using a Bone Substitute Supported by Mesenchymal Stem Cells Derived from the Umbilical Cord

Author:

Kosinski Michal1ORCID,Figiel-Dabrowska Anna1,Lech Wioletta2,Wieprzowski Lukasz3,Strzalkowski Ryszard4,Strzemecki Damian5,Cheda Lukasz6,Lenart Jacek7,Domanska-Janik Krystyna2ORCID,Sarnowska Anna1ORCID

Affiliation:

1. Translational Platform for Regenerative Medicine, Mossakowski Medical Research Centre, Polish Academy of Sciences, Poland

2. Department of Stem Cell Bioengineering, Mossakowski Medical Research Centre, Polish Academy of Sciences, Poland

3. Paediatric Surgery Clinic, Institute of Mother and Child, Poland

4. Electron Microscopy Platform, Mossakowski Medical Research Centre, Polish Academy of Sciences, Poland

5. Department of Experimental Pharmacology, Mossakowski Medical Research Centre, Polish Academy of Sciences, Poland

6. Faculty of Chemistry, Biological and Chemical Research Centre, University of Warsaw, Poland

7. Department of Neurochemistry, Mossakowski Medical Research Centre, Polish Academy of Sciences, Poland

Abstract

Objective. Bone defects or atrophy may arise as a consequence of injury, inflammation of various etiologies, and neoplastic or traumatic processes or as a result of surgical procedures. Sometimes the regeneration process of bone loss is impaired, significantly slowed down, or does not occur, e.g., in congenital defects. For the bone defect reconstruction, a piece of the removed bone from ala of ilium or bone transplantation from a decedent is used. Replacement of the autologous or allogenic source of the bone-by-bone substitute could reduce the number of surgeries and time in the pharmacological coma during the reconstruction of the bone defect. Application of mesenchymal stem cells in the reconstruction surgery may have positive influence on tissue regeneration by secretion of angiogenic factors, recruitment of other MSCs, or differentiation into osteoblasts.Materials and Methods. Mesenchymal stem cells derived from the umbilical cord (Wharton’s jelly (WJ-MSC)) were cultured in GMP-grade DMEM low glucose supplemented with heparin, 10% platelet lysate, glucose, and antibiotics.In vitroWJ-MSCs were seeded on the bone substitute Bio-Oss Collagen® and cultured in the StemPro® Osteogenesis Differentiation Kit. During the culture on the 1st, 7th, 14th, and 21st day (day in vitro (DIV)), we analyzed viability (confocal microscopy) and adhesion capability (electron microscopy) of WJ-MSC on Bio-Oss scaffolds, gene expression (qPCR), and secretion of proteins (Luminex).In vivoBio-Oss® scaffolds with WJ-MSC were transplanted to trepanation holes in the cranium to obtain their overgrowth. The computed tomography was performed 7, 14, and 21 days after surgery to assess the regeneration.Results. The Bio-Oss® scaffold provides a favourable environment for WJ-MSC survival. WJ-MSCs in osteodifferentiation medium are able to attach and proliferate on Bio-Oss® scaffolds. Results obtained from qPCR and Luminex® indicate that WJ-MSCs possess the ability to differentiate into osteoblast-like cells and may induce osteoclastogenesis, angiogenesis, and mobilization of host MSCs. In animal studies, WJ-MSCs seeded on Bio-Oss® increased the scaffold integration with host bone and changed their morphology to osteoblast-like cells.Conclusions. The presented construct consisted of Bio-Oss®, the scaffold with high flexibility and plasticity, approved for clinical use with seeded immunologically privileged WJ-MSC which may be considered reconstructive therapy in bone defects.

Funder

National Centre for Research and Development

Publisher

Hindawi Limited

Subject

Cell Biology,Molecular Biology

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