Is Transcatheter Aortic Valve Implantation of Living Tissue-Engineered Valves Feasible? An In Vitro Evaluation Utilizing a Decellularized and Reseeded Biohybrid Valve

Fabian Koenig; Jang-Sun Lee; Bassil Akra; Trixi Hollweck; Erich Wintermantel; Christian Hagl; Nikolaus Thierfelder

doi:10.1111/aor.12683

Is Transcatheter Aortic Valve Implantation of Living Tissue-Engineered Valves Feasible? An In Vitro Evaluation Utilizing a Decellularized and Reseeded Biohybrid Valve

Artif Organs. 2016 Aug;40(8):727-37. doi: 10.1111/aor.12683. Epub 2016 May 17.

Authors

Fabian Koenig^{1

2}, Jang-Sun Lee¹, Bassil Akra¹, Trixi Hollweck¹, Erich Wintermantel², Christian Hagl¹, Nikolaus Thierfelder¹

Affiliations

¹ Department of Cardiac Surgery, Laboratory for Tissue Engineering, Grosshadern Medical Centre, Ludwig Maximilians University, Munich.
² Department of Medical Engineering, Technical University Munich, Garching, Germany.

PMID: 27187768
DOI: 10.1111/aor.12683

Abstract

Transcatheter aortic valve implantation (TAVI) is a fast-growing, exciting field of invasive therapy. During the last years many innovations significantly improved this technique. However, the prostheses are still associated with drawbacks. The aim of this study was to create cell-seeded biohybrid aortic valves (BAVs) as an ideal implant by combination of assets of biological and artificial materials. Furthermore, the influence of TAVI procedure on tissue-engineered BAV was investigated. BAV (n=6) were designed with decellularized homograft cusps and polyurethane walls. They were seeded with fibroblasts and endothelial cells isolated from saphenous veins. Consecutively, BAV were conditioned under low pulsatile flow (500 mL/min) for 5 days in a specialized bioreactor. After conditioning, TAVI-simulation was performed. The procedure was concluded with re-perfusion of the BAV for 2 days at an increased pulsatile flow (1100 mL/min). Functionality was assessed by video-documentation. Samples were taken after each processing step and evaluated by scanning electron microscopy (SEM), immunohistochemical staining (IHC), and Live/Dead-assays. The designed BAV were fully functioning and displayed physiologic behavior. After cell seeding, static cultivation and first conditioning, confluent cell layers were observed in SEM. Additionally, IHC indicated the presence of endothelial cells and fibroblasts. A significant construction of extracellular matrix was detected after the conditioning phase. However, a large number of lethal cells were observed after crimping by Live/Dead staining. Analysis revealed that the cells while still being present directly after crimping were removed in subsequent perfusion. Extensive regions of damaged cell-layers were detected by SEM-analysis substantiating these findings. Furthermore, increased ICAM expression was detected after re-perfusion as manifestation of inflammatory reaction. The approach to generate biohybrid valves is promising. However, damages inflicted during the crimping process seem not to be immediately detectable. Due to severe impacts on seeded cells, the strategy of living TE valves for TAVI should be reconsidered.

Keywords: Cardiovascular tissue engineering-Aortic valve-Decellularization-Transcatheter aortic valve implantation-Homografts-Bioreactor.

MeSH terms

Aortic Valve / cytology
Aortic Valve / surgery*
Bioprosthesis*
Bioreactors
Cells, Cultured
Endothelial Cells / cytology
Equipment Design
Fibroblasts / cytology
Heart Valve Prosthesis*
Humans
Polyurethanes / chemistry
Saphenous Vein / cytology
Tissue Engineering / methods*
Tissue Scaffolds / chemistry
Transcatheter Aortic Valve Replacement*

Substances

Polyurethanes