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A combined physicochemical approach towards human tenocyte phenotype maintenance.

作者信息

Ryan C N M, Pugliese E, Shologu N, Gaspar D, Rooney P, Islam Md N, O'Riordan A, Biggs M J, Griffin M D, Zeugolis D I

机构信息

Regenerative, Modular & Developmental Engineering Laboratory (REMODEL), Biomedical Sciences Building, National University of Ireland Galway (NUI Galway), Galway, Ireland.

Science Foundation Ireland (SFI) Centre for Research in Medical Devices (CÚRAM), Biomedical Sciences Building, National University of Ireland Galway (NUI Galway), Galway, Ireland.

出版信息

Mater Today Bio. 2021 Sep 10;12:100130. doi: 10.1016/j.mtbio.2021.100130. eCollection 2021 Sep.


DOI:10.1016/j.mtbio.2021.100130
PMID:34632361
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8488312/
Abstract

During culture, bereft of their optimal tissue context, tenocytes lose their phenotype and function. Considering that tenocytes in their native tissue milieu are exposed simultaneously to manifold signals, combination approaches (e.g. growth factor supplementation and mechanical stimulation) are continuously gaining pace to control cell fate during expansion, albeit with limited success due to the literally infinite number of possible permutations. In this work, we assessed the potential of scalable and potent physicochemical approaches that control cell fate (substrate stiffness, anisotropic surface topography, collagen type I coating) and enhance extracellular matrix deposition (macromolecular crowding) in maintaining human tenocyte phenotype in culture. Cell morphology was primarily responsive to surface topography. The tissue culture plastic induced the largest nuclei area, the lowest aspect ratio, and the highest focal adhesion kinase. Collagen type I coating increased cell number and metabolic activity. Cell viability was not affected by any of the variables assessed. Macromolecular crowding intensely enhanced and accelerated native extracellular matrix deposition, albeit not in an aligned fashion, even on the grooved substrates. Gene analysis at day 14 revealed that the 130 kPa grooved substrate without collagen type I coating and under macromolecular crowding conditions positively regulated human tenocyte phenotype. Collectively, this work illustrates the beneficial effects of combined physicochemical approaches in controlling cell fate during expansion.

摘要

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本文引用的文献

[1]
Growth factor and macromolecular crowding supplementation in human tenocyte culture.

Biomater Biosyst. 2021-1-30

[2]
Collagen type II: From biosynthesis to advanced biomaterials for cartilage engineering.

Biomater Biosyst. 2021-11-22

[3]
It is time to crowd your cell culture media - Physicochemical considerations with biological consequences.

Biomaterials. 2021-8

[4]
Transforming eukaryotic cell culture with macromolecular crowding.

Trends Biochem Sci. 2021-10

[5]
Hyaluronic Acid as Macromolecular Crowder in Equine Adipose-Derived Stem Cell Cultures.

Cells. 2021-4-9

[6]
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NPJ Regen Med. 2021-3-29

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Cell derived extracellular matrix-rich biomimetic substrate supports podocyte proliferation, differentiation and maintenance of native phenotype.

Adv Funct Mater. 2020-10-28

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Am J Physiol Cell Physiol. 2021-5-1

[9]
Multi-omic single cell analysis resolves novel stromal cell populations in healthy and diseased human tendon.

Sci Rep. 2020-9-3

[10]
Seaweed polysaccharides as macromolecular crowding agents.

Int J Biol Macromol. 2020-12-1

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