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Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair

[Image: see text] Tubular scaffolds which incorporate a variety of micro- and nanotopographies have a wide application potential in tissue engineering especially for the repair of spinal cord injury (SCI). We aim to produce metabolically active differentiated tissues within such tubes, as it is cruc...

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Autores principales: Donoghue, Peter S., Sun, Tao, Gadegaard, Nikolaj, Riehle, Mathis O., Barnett, Susan C.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2013
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4087043/
https://www.ncbi.nlm.nih.gov/pubmed/24279373
http://dx.doi.org/10.1021/mp400526n
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author Donoghue, Peter S.
Sun, Tao
Gadegaard, Nikolaj
Riehle, Mathis O.
Barnett, Susan C.
author_facet Donoghue, Peter S.
Sun, Tao
Gadegaard, Nikolaj
Riehle, Mathis O.
Barnett, Susan C.
author_sort Donoghue, Peter S.
collection PubMed
description [Image: see text] Tubular scaffolds which incorporate a variety of micro- and nanotopographies have a wide application potential in tissue engineering especially for the repair of spinal cord injury (SCI). We aim to produce metabolically active differentiated tissues within such tubes, as it is crucially important to evaluate the biological performance of the three-dimensional (3D) scaffold and optimize the bioprocesses for tissue culture. Because of the complex 3D configuration and the presence of various topographies, it is rarely possible to observe and analyze cells within such scaffolds in situ. Thus, we aim to develop scaled down mini-chambers as simplified in vitro simulation systems, to bridge the gap between two-dimensional (2D) cell cultures on structured substrates and three-dimensional (3D) tissue culture. The mini-chambers were manipulated to systematically simulate and evaluate the influences of gravity, topography, fluid flow, and scaffold dimension on three exemplary cell models that play a role in CNS repair (i.e., cortical astrocytes, fibroblasts, and myelinating cultures) within a tubular scaffold created by rolling up a microstructured membrane. Since we use CNS myelinating cultures, we can confirm that the scaffold does not affect neural cell differentiation. It was found that heterogeneous cell distribution within the tubular constructs was caused by a combination of gravity, fluid flow, topography, and scaffold configuration, while cell survival was influenced by scaffold length, porosity, and thickness. This research demonstrates that the mini-chambers represent a viable, novel, scale down approach for the evaluation of complex 3D scaffolds as well as providing a microbioprocessing strategy for tissue engineering and the potential repair of SCI.
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spelling pubmed-40870432014-07-09 Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair Donoghue, Peter S. Sun, Tao Gadegaard, Nikolaj Riehle, Mathis O. Barnett, Susan C. Mol Pharm [Image: see text] Tubular scaffolds which incorporate a variety of micro- and nanotopographies have a wide application potential in tissue engineering especially for the repair of spinal cord injury (SCI). We aim to produce metabolically active differentiated tissues within such tubes, as it is crucially important to evaluate the biological performance of the three-dimensional (3D) scaffold and optimize the bioprocesses for tissue culture. Because of the complex 3D configuration and the presence of various topographies, it is rarely possible to observe and analyze cells within such scaffolds in situ. Thus, we aim to develop scaled down mini-chambers as simplified in vitro simulation systems, to bridge the gap between two-dimensional (2D) cell cultures on structured substrates and three-dimensional (3D) tissue culture. The mini-chambers were manipulated to systematically simulate and evaluate the influences of gravity, topography, fluid flow, and scaffold dimension on three exemplary cell models that play a role in CNS repair (i.e., cortical astrocytes, fibroblasts, and myelinating cultures) within a tubular scaffold created by rolling up a microstructured membrane. Since we use CNS myelinating cultures, we can confirm that the scaffold does not affect neural cell differentiation. It was found that heterogeneous cell distribution within the tubular constructs was caused by a combination of gravity, fluid flow, topography, and scaffold configuration, while cell survival was influenced by scaffold length, porosity, and thickness. This research demonstrates that the mini-chambers represent a viable, novel, scale down approach for the evaluation of complex 3D scaffolds as well as providing a microbioprocessing strategy for tissue engineering and the potential repair of SCI. American Chemical Society 2013-11-26 2014-07-07 /pmc/articles/PMC4087043/ /pubmed/24279373 http://dx.doi.org/10.1021/mp400526n Text en Copyright © 2013 American Chemical Society Terms of Use (http://pubs.acs.org/page/policy/authorchoice_termsofuse.html)
spellingShingle Donoghue, Peter S.
Sun, Tao
Gadegaard, Nikolaj
Riehle, Mathis O.
Barnett, Susan C.
Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title_full Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title_fullStr Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title_full_unstemmed Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title_short Development of a Novel 3D Culture System for Screening Features of a Complex Implantable Device for CNS Repair
title_sort development of a novel 3d culture system for screening features of a complex implantable device for cns repair
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4087043/
https://www.ncbi.nlm.nih.gov/pubmed/24279373
http://dx.doi.org/10.1021/mp400526n
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