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Tytuł pozycji:

Artificial decellularized extracellular matrix improves the regenerative capacity of adipose tissue derived stem cells on 3D printed polycaprolactone scaffolds

Tytuł:
Artificial decellularized extracellular matrix improves the regenerative capacity of adipose tissue derived stem cells on 3D printed polycaprolactone scaffolds
Autorzy:
Jana C Blum
Thilo L Schenck
Alexandra Birt
Riccardo E Giunta
Paul S Wiggenhauser
Temat:
Biochemistry
QD415-436
Źródło:
Journal of Tissue Engineering, Vol 12 (2021)
Wydawca:
SAGE Publishing, 2021.
Rok publikacji:
2021
Kolekcja:
LCC:Biochemistry
Typ dokumentu:
article
Opis pliku:
electronic resource
Język:
English
ISSN:
2041-7314
20417314
Relacje:
https://doaj.org/toc/2041-7314
DOI:
10.1177/20417314211022242
Dostęp URL:
https://doaj.org/article/e98cae6d2380449ca2ae7d8523db4ed1  Link otwiera się w nowym oknie
Numer akcesji:
edsdoj.98cae6d2380449ca2ae7d8523db4ed1
Czasopismo naukowe
Ideal tissue engineering frameworks should be both an optimal biological microenvironment and a shape and stability providing framework. In this study we tried to combine the advantages of cell-derived artificial extracellular matrix (ECM) with those of 3D printed polycaprolactone (PCL) scaffolds. In Part A, both chondrogenic and osteogenic ECMs were produced by human adipose derived stem cells (hASCs) on 3D-printed PCL scaffolds and then decellularized to create cell free functionalized PCL scaffolds, named acPCL and aoPCL respectively. The decellularization resulted in a significant reduction of the DNA content as well as the removal of nuclei while the ECM was largely preserved. In Part B the bioactivation and the effect of the ac/aoPCL scaffolds on the proliferation, differentiation, and gene expression of hASCs was investigated. The ac/aoPCL scaffolds were found to be non-toxic and allow good adhesion, but do not affect proliferation. In the in vitro investigation of cartilage regeneration, biochemical analysis showed that acPCL scaffolds have an additional effect on chondrogenic differentiation as gene expression analysis showed markers of cartilage hypertrophy. The aoPCL showed a large influence on the differentiation of hASCs. In control medium they were able to stimulate hASCs to produce calcium alone and all genes relevant investigated for osteogenesis were significantly higher expressed on aoPCL than on unmodified PCL. Therefore, we believe that ac/aoPCL scaffolds have a high potential to improve regenerative capacity of unmodified PCL scaffolds and should be further investigated.
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