Development and In Vitro/In Vivo Comparative Characterization of Cryopreserved and Decellularized Tracheal Grafts

Author:

Stocco Elena123,Barbon Silvia123ORCID,Mammana Marco24,Trojan Diletta5ORCID,Bianchin Alice5,Favaretto Francesca5,Contran Martina1,Zambello Giovanni4,Vogliardi Andrea6ORCID,Confalonieri Marta7ORCID,Todros Silvia7ORCID,Pavan Piero G.78,Romanato Filippo26ORCID,Conconi Maria Teresa9,Macchi Veronica123ORCID,De Caro Raffaele123ORCID,Rea Federico24,Porzionato Andrea123

Affiliation:

1. Section of Human Anatomy, Department of Neuroscience, University of Padova, 35121 Padova, Italy

2. L.i.f.e.L.a.b. Program, Consorzio per la Ricerca Sanitaria (CORIS), Veneto Region, 35128 Padova, Italy

3. Foundation for Biology and Regenerative Medicine, Tissue Engineering and Signaling-TES, Onlus, 35136 Padova, Italy

4. Thoracic Surgery Division, Department of Cardiac, Thoracic, Vascular Sciences and Public Health, Padova University Hospital, Via Giustiniani, 2, 35128 Padova, Italy

5. Tissue Bank, Fondazione Banca dei Tessuti del Veneto ETS, 31100 Treviso, Italy

6. Department of Physics and Astronomy ‘G. Galilei’, University of Padova, 35131 Padova, Italy

7. Department of Industrial Engineering, University of Padova, 35131 Padova, Italy

8. Fondazione Istituto di Ricerca Pediatrica Città della Speranza, 35127 Padova, Italy

9. Department of Pharmaceutical and Pharmacological Sciences, University of Padova, 35131 Padova, Italy

Abstract

Tracheal reconstruction represents a challenge when primary anastomosis is not feasible. Within this scenario, the study aim was to develop a new pig-derived decellularized trachea (DecellT) to be compared with the cryopreserved counterpart (CryoT) for a close predictive analysis. Tracheal segments underwent decellularization by a physical + enzymatic + chemical method (12 cycles); in parallel, cryopreserved samples were also prepared. Once decellularized (histology/DNA quantification), the two groups were characterized for Alpha-Gal epitopes/structural proteins (immunohistochemistry/histology/biochemical assays/second harmonic generation microscopy)/ultrastructure (Scanning Electron Microscopy (SEM))/mechanical behaviour. Cytotoxicity absence was assessed in vitro (extract-test assay/direct seeding, HM1SV40 cell line) while biocompatibility was verified in BALB/c mice, followed by histological/immunohistochemical analyses and SEM (14 days). Decellularization effectively removed Alpha-Gal epitopes; cartilage histoarchitecture was retained in both groups, showing chondrocytes only in the CryoT. Cryopreservation maintained few respiratory epithelium sparse cilia, not detectable in DecellT. Focusing on ECM, preserved structural/ultrastructural organization and collagen content were observed in the cartilage of both; conversely, the GAGs were significantly reduced in DecellT, as confirmed by mechanical study results. No cytotoxicity was highlighted by CryoT/DecellT in vitro, as they were also corroborated by a biocompatibility assay. Despite some limitations (cells presence/GAGs reduction), CryoT/DecellT are both appealing options, which warrant further investigation in comparative in vivo studies.

Funder

‘Consorzio per la Ricerca Sanitaria’

Publisher

MDPI AG

Subject

General Medicine

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