Quantifying extracellular matrix turnover in human lung scaffold cultures
Rosmark, Oskar LU
; Åhrman, Emma
LU
; Müller, Catharina
LU
; Elowsson Rendin, Linda
LU
; Eriksson, Leif
LU
; Malmström, Anders
LU
; Hallgren, Oskar
LU
; Larsson-Callerfelt, Anna Karin
LU
; Westergren-Thorsson, Gunilla
LU
and Malmström, Johan
LU
(2018)
In Scientific Reports
8(1).
- Abstract
Remodelling of the extracellular matrix is accomplished by altering the balance between matrix macromolecule production and degradation. However, it is not well understood how cells balance production of new matrix molecules and degradation of existing ones during tissue remodelling and regeneration. In this study, we used decellularized lung scaffolds repopulated with allogenic lung fibroblasts cultured with stable isotope labelled amino acids to quantify the balance between matrix production and degradation at a proteome-wide scale. Specific temporal dynamics of different matrisome proteins were found to correspond to the proliferative activity of the repopulating cells and the degree of extracellular deposition. The remodeling of the... (More)
Remodelling of the extracellular matrix is accomplished by altering the balance between matrix macromolecule production and degradation. However, it is not well understood how cells balance production of new matrix molecules and degradation of existing ones during tissue remodelling and regeneration. In this study, we used decellularized lung scaffolds repopulated with allogenic lung fibroblasts cultured with stable isotope labelled amino acids to quantify the balance between matrix production and degradation at a proteome-wide scale. Specific temporal dynamics of different matrisome proteins were found to correspond to the proliferative activity of the repopulating cells and the degree of extracellular deposition. The remodeling of the scaffold was characterized by an initial phase with cell proliferation and high production of cell adhesion proteins such as emilin-1 and fibronectin. Extended culture time resulted in increased levels of core matrisome proteins. In a comparison with monolayer cultures on plastic, culture in lung scaffolds lead to a pronounced accumulation of proteoglycans, such as versican and decorin, resulting in regeneration of an extracellular matrix with greater resemblance to native lung tissue compared to standard monolayer cultures. Collectively, the study presents a promising technique for increasing the understanding of cell- extracellular matrix interactions under healthy and diseased conditions.
(Less)
- author
- Rosmark, Oskar
LU
; Åhrman, Emma
LU
; Müller, Catharina
LU
; Elowsson Rendin, Linda
LU
; Eriksson, Leif
LU
; Malmström, Anders
LU
; Hallgren, Oskar
LU
; Larsson-Callerfelt, Anna Karin
LU
; Westergren-Thorsson, Gunilla
LU
and Malmström, Johan
LU
- organization
- publishing date
- 2018-12-01
- type
- Contribution to journal
- publication status
- published
- subject
- in
- Scientific Reports
- volume
- 8
- issue
- 1
- article number
- 5409
- publisher
- Nature Publishing Group
- external identifiers
-
- scopus:85044953122
- pmid:29615673
- ISSN
- 2045-2322
- DOI
- 10.1038/s41598-018-23702-x
- language
- English
- LU publication?
- yes
- id
- 7676945c-728e-4e6e-b460-d1677b24934b
- date added to LUP
- 2018-04-16 15:09:35
- date last changed
- 2024-02-13 18:54:59
@article{7676945c-728e-4e6e-b460-d1677b24934b,
abstract = {{<p>Remodelling of the extracellular matrix is accomplished by altering the balance between matrix macromolecule production and degradation. However, it is not well understood how cells balance production of new matrix molecules and degradation of existing ones during tissue remodelling and regeneration. In this study, we used decellularized lung scaffolds repopulated with allogenic lung fibroblasts cultured with stable isotope labelled amino acids to quantify the balance between matrix production and degradation at a proteome-wide scale. Specific temporal dynamics of different matrisome proteins were found to correspond to the proliferative activity of the repopulating cells and the degree of extracellular deposition. The remodeling of the scaffold was characterized by an initial phase with cell proliferation and high production of cell adhesion proteins such as emilin-1 and fibronectin. Extended culture time resulted in increased levels of core matrisome proteins. In a comparison with monolayer cultures on plastic, culture in lung scaffolds lead to a pronounced accumulation of proteoglycans, such as versican and decorin, resulting in regeneration of an extracellular matrix with greater resemblance to native lung tissue compared to standard monolayer cultures. Collectively, the study presents a promising technique for increasing the understanding of cell- extracellular matrix interactions under healthy and diseased conditions.</p>}},
author = {{Rosmark, Oskar and Åhrman, Emma and Müller, Catharina and Elowsson Rendin, Linda and Eriksson, Leif and Malmström, Anders and Hallgren, Oskar and Larsson-Callerfelt, Anna Karin and Westergren-Thorsson, Gunilla and Malmström, Johan}},
issn = {{2045-2322}},
language = {{eng}},
month = {{12}},
number = {{1}},
publisher = {{Nature Publishing Group}},
series = {{Scientific Reports}},
title = {{Quantifying extracellular matrix turnover in human lung scaffold cultures}},
url = {{http://dx.doi.org/10.1038/s41598-018-23702-x}},
doi = {{10.1038/s41598-018-23702-x}},
volume = {{8}},
year = {{2018}},
}