Adipose-derived stromal cells increase the formation of collagens through paracrine and juxtacrine mechanisms in a fibroblast co-culture model utilizing macromolecular crowding

Rebekka Harary Søndergaard; Lisbeth Drozd Højgaard; Alexander Lynge Reese-Petersen; Cecilie Hoeeg; Anders Bruun Mathiasen; Mandana Haack-Sørensen; Bjarke Follin; Federica Genovese; Jens Kastrup; Morten Juhl; Annette Ekblond

doi:10.1186/s13287-022-02923-y

Adipose-derived stromal cells increase the formation of collagens through paracrine and juxtacrine mechanisms in a fibroblast co-culture model utilizing macromolecular crowding

Stem Cell Res Ther. 2022 Jun 11;13(1):250. doi: 10.1186/s13287-022-02923-y.

Affiliations

¹ Cardiology Stem Cell Centre, The Heart Centre, Copenhagen University Hospital Rigshospitalet, Henrik Harpestrengs vej 4C, Dept. 9302, 2100, Copenhagen, Denmark. rebekka.harary.soendergaard@regionh.dk.
² Cardiology Stem Cell Centre, The Heart Centre, Copenhagen University Hospital Rigshospitalet, Henrik Harpestrengs vej 4C, Dept. 9302, 2100, Copenhagen, Denmark.
³ Nordic Bioscience A/S, Herlev Hovedgade 205-207, 2730, Herlev, Denmark.
⁴ Department of Cardiology, The Heart Centre, Copenhagen University Hospital Rigshospitalet, Blegdamsvej 9, 2100, Copenhagen, Denmark.

Abstract

Background: Adipose-derived stromal cells (ASCs) possess a multitude of regenerative capabilities, which include immunomodulation, angiogenesis, and stimulation of extracellular matrix (ECM) remodeling. However, the underlying mechanisms leading to ECM remodeling remain largely elusive and highlight the need for functional in vitro models for mode of action studies. Therefore, the purpose of this study was to develop an in vitro co-culture model to investigate the capabilities of ASCs to modulate fibroblasts and ECM.

Methods: An ECM in vitro model with ASCs and normal human dermal fibroblasts (NHDFs) was established utilizing macromolecular crowding, ascorbic acid, and TGF-β stimulation. Paracrine and juxtacrine co-cultures were created using transwell inserts and cell cultures with direct cell-cell contacts. The cultures were screened using RT² PCR Profiler Arrays; the protein levels of myofibroblast differentiation marker alpha smooth muscle actin (αSMA) and ECM remodeling enzymes were analyzed using western blot on cell lysates; the formation of collagen type I, III, VI, and fibronectin was investigated using ELISA on culture supernatants; and the deposition of collagens was analyzed using immunocytochemistry.

Results: TGF-β stimulation of NHDF monocultures increased the expression of 18 transcripts relevant for ECM formation and remodeling, the protein levels of αSMA and matrix metalloproteinase-2 (MMP-2), the formation of collagen type I, III, VI, and fibronectin, and the deposition of collagen type I and VI and decreased the protein levels of MMP-14. Inclusion of ASCs in the ECM co-culture model increased the formation of collagen type I and III through paracrine mechanisms and the formation of collagen type VI through juxtacrine mechanisms.

Conclusions: The co-culture model provides effective stimulation of NHDF monocultures by TGF-β for enhanced formation and deposition of ECM. In the model, ASCs induce changes in ECM by increasing formation of collagen type I, III and VI. The obtained results could guide further investigations of ASCs' capabilities and underlying mechanisms related to ECM formation and remodeling.

Keywords: Adipose-derived stromal cells; Extracellular matrix; Fibroblasts; Macromolecular crowding; Metalloproteinases; Paracrine and juxtacrine co-cultures.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cells, Cultured
Coculture Techniques
Collagen / metabolism
Collagen Type I / metabolism
Extracellular Matrix / metabolism
Fibroblasts
Fibronectins* / metabolism
Humans
Matrix Metalloproteinase 2* / genetics
Matrix Metalloproteinase 2* / metabolism
Stromal Cells / metabolism
Transforming Growth Factor beta / metabolism

Substances

Collagen Type I
Fibronectins
Transforming Growth Factor beta
Collagen
Matrix Metalloproteinase 2