Optimized Decellularization of a Porcine Fasciocutaneaous Flap

Author:

Lupon Elise123ORCID,Acun Aylin345,Taveau Corentin B.23,Oganesyan Ruben34ORCID,Lancia Hyshem H.26ORCID,Andrews Alec R.23,Randolph Mark A.23,Cetrulo Curtis L.237,Lellouch Alexandre G.238ORCID,Uygun Basak E.34

Affiliation:

1. Department of Plastic and Reconstructive Surgery, Institut Universitaire Locomoteur et du Sport, Pasteur 2 Hospital, University Côte d’Azur, 06300 Nice, France

2. Vascularized Composite Allotransplantation Laboratory, Center for Transplantation Sciences, Massachusetts General Hospital, Harvard Medical School, Boston, MA 02114, USA

3. Shriners Children’s Boston, Boston, MA 02114, USA

4. Center for Engineering in Medicine and Surgery, Massachusetts General Hospital, Harvard Medical School, Boston, MA 02114, USA

5. Department of Biomedical Engineering, Widener University, Chester, PA 19013, USA

6. University of Grenoble Alpes, CNRS, TIMC UMR 5525, EPSP, 38000 Grenoble, France

7. Department of Plastic and Reconstructive Surgery, Massachusetts General Hospital, Boston, MA 02114, USA

8. Innovative Therapies in Haemostasis, INSERM UMR-S 1140, University of Paris, 75015 Paris, France

Abstract

Reconstructive techniques to repair severe tissue defects include the use of autologous fasciocutaneous flaps, which may be limited due to donor site availability or lead to complications such as donor site morbidity. A number of synthetic or natural dermal substitutes are in use clinically, but none have the architectural complexity needed to reconstruct deep tissue defects. The perfusion decellularization of fasciocutaneous flaps is an emerging technique that yields a scaffold with the necessary composition and vascular microarchitecture and serves as an alternative to autologous flaps. In this study, we show the perfusion decellularization of porcine fasciocutaneous flaps using sodium dodecyl sulfate (SDS) at three different concentrations, and identify that 0.2% SDS results in a decellularized flap that is efficiently cleared of its cellular material at 86%, has maintained its collagen and glycosaminoglycan content, and preserved its microvasculature architecture. We further demonstrate that the decellularized graft has the porous structure and growth factors that would facilitate repopulation with cells. Finally, we show the biocompatibility of the decellularized flap using human dermal fibroblasts, with cells migrating as deep as 150 µm into the tissue over a 7-day culture period. Overall, our results demonstrate the promise of decellularized porcine flaps as an interesting alternative for reconstructing complex soft tissue defects, circumventing the limitations of autologous skin flaps.

Funder

Shriners Hospitals for Children

National Institutes of Health/The National Institute of Arthritis and Musculoskeletal and Skin Diseases

Shriners Children’s

La Bourse des Gueules Cassées

La fondation de la vocation

Shriners Special Shared Facilities Translational Regenerative Medicine

Morphology and Imaging

Genomics and Proteomics

Publisher

MDPI AG

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