Mesenchymal Stromal Cell-Seeded Biomimetic Scaffolds as a Factory of Soluble RANKL in Rankl-Deficient Osteopetrosis

Author:

Menale Ciro12,Campodoni Elisabetta3,Palagano Eleonora24,Mantero Stefano12,Erreni Marco2,Inforzato Antonio24,Fontana Elena12,Schena Francesca5,van’t Hof Rob6,Sandri Monica3,Tampieri Anna3,Villa Anna12,Sobacchi Cristina12

Affiliation:

1. CNR-IRGB, Milan Unit, Milan, Italy

2. Humanitas Clinical and Research Institute, Rozzano, Italy

3. CNR-ISTEC, Faenza, Italy

4. Department of Medical Biotechnologies and Translational Medicine University of Milan, Milan, Italy

5. Clinica Pediatrica e Reumatologia UOSD Centro Malattie Autoinfiammatorie e Immunodeficienze, Genoa, Italy

6. Bone Research Group, Institute of Ageing & Chronic Disease University of Liverpool, Liverpool, UK

Abstract

Abstract Biomimetic scaffolds are extremely versatile in terms of chemical composition and physical properties, which can be defined to accomplish specific applications. One property that can be added is the production/release of bioactive soluble factors, either directly from the biomaterial, or from cells embedded within the biomaterial. We reasoned that pursuing this strategy would be appropriate to setup a cell-based therapy for RANKL-deficient autosomal recessive osteopetrosis, a very rare skeletal genetic disease in which lack of the essential osteoclastogenic factor RANKL impedes osteoclast formation. The exogenously administered RANKL cytokine is effective in achieving osteoclast formation and function in vitro and in vivo, thus, we produced murine Rankl−/− mesenchymal stromal cells (MSCs) overexpressing human soluble RANKL (hsRL) following lentiviral transduction (LVhsRL). Here, we described a three-dimensional (3D) culture system based on a magnesium-doped hydroxyapatite/collagen I (MgHA/Col) biocompatible scaffold closely reproducing bone physicochemical properties. MgHA/Col-seeded murine MSCs showed improved properties, as compared to two-dimensional (2D) culture, in terms of proliferation and hsRL production, with respect to LVhsRL-transduced cells. When implanted subcutaneously in Rankl−/− mice, these cell constructs were well tolerated, colonized by host cells, and intensely vascularized. Of note, in the bone of Rankl−/− mice that carried scaffolds with either WT or LVhsRL-transduced Rankl−/− MSCs, we specifically observed formation of TRAP+ cells, likely due to sRL released from the scaffolds into circulation. Thus, our strategy proved to have the potential to elicit an effect on the bone; further work is required to maximize these benefits and achieve improvements of the skeletal pathology in the treated Rankl−/− mice. Stem Cells Translational Medicine  2019;8:22–34

Funder

European Community’s Seventh Framework Program

PRIN Project

Programma Nazionale per la Ricerca-Consiglio Nazionale delle Ricerche Aging Project

Ministero della Salute

Fondazione Nicola Del Roscio

Publisher

Oxford University Press (OUP)

Subject

Cell Biology,Developmental Biology,General Medicine

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