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Native and decellularized porcine vena cava: Histological analysis and in vitro repopulation

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Author
Massaro, Maria StefaniaORCiD Profile - 0000-0001-6146-1116Scopus Profile - 57224086072
Pálek, RichardORCiD Profile - 0000-0002-3546-808XScopus Profile - 56056174600
Malečková, AnnaORCiD Profile - 0000-0003-2674-6268WoS Profile - R-2499-2017Scopus Profile - 55993410700
Grajciarová, Martina
Červenková, Lenka
Polák, Robert
Šarčević, SimaScopus Profile - 58097707900
Ševčík, Jan
Bolek, Lukáš
Tonar, ZbyněkORCiD Profile - 0000-0002-7200-9894WoS Profile - I-2728-2017Scopus Profile - 24279165900
Liška, VáclavORCiD Profile - 0000-0002-5226-0280WoS Profile - Q-4402-2017Scopus Profile - 8705914800
Moulisová, VladimíraORCiD Profile - 0000-0003-0700-2837Scopus Profile - 14056600500

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Publication date
2025
Published in
Biomaterials Advances
Volume / Issue
177 (December)
ISBN / ISSN
ISSN: 2772-9508
ISBN / ISSN
eISSN: 2772-9508
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  • Faculty of Medicine in Pilsen

This publication has a published version with DOI 10.1016/j.bioadv.2025.214382

Abstract
Current standards in vascular reconstruction imply the use of autologous or synthetic material. Despite being standard, autologous grafts are limited by pathologies already affecting the patient and possible complications at the site of explantation, while synthetic grafts carry increased infection risks. Decellularized tissues have gained significant attention due to their potential for improving integration and functionality. The decellularization process removes cellular components while retaining the extracellular matrix, providing a scaffold that supports endothelial cell growth and minimizes immune rejection. Porcine decellularized vena cava is a promising candidate for vascular graft applications due to its structural similarity to human blood vessels and biocompatibility. In this study, we decellularized porcine vena cava with a combination of Triton X-100 and sodium dodecyl sulfate in four hours. We subsequently characterized the wall structure through histological stainings and proteomic analysis. Parameters such as wall thickness, intima-media layers thickness, collagen and elastin area fraction were quantified and compared. Moreover, decellularized veins were repopulated in vitro with human endothelial cells in static and dynamic conditions to verify the adhesion of human cells to the porcine scaffold and fully functionalize the lumen. An in-house-designed bioreactor was developed to seed endothelial cells on the lumen, mimicking the in vivo blood flow.
Keywords
Decellularization, Porcine vena cava, Histological analysis, Proteomics, Bioreactor repopulation
Permanent link
https://hdl.handle.net/20.500.14178/3138
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WOS:001513422000002
SCOPUS:2-s2.0-105008201416
PUBMED:40532651
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Full text of this result is licensed under: Creative Commons Uveďte původ 4.0 International

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