Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture

Although conventional two-dimensional (2D) cell culture is convenient for routine work, researchers are turning to three-dimensional (3D) cell culture for more accurate, physiologically representative information on the way their cells behave and respond to stimuli. Cells can now be routinely cultur...

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Bibliographic Details
Main Author: Rossouw, C.L. (Claire Louise)
Other Authors: Moolman, Samantha
Published: 2013
Subjects:
Online Access:http://hdl.handle.net/2263/24273
Rossouw, CL 2013, Development and applications of a novel, hermoresponsive scaffold for three-dimensional cell culture, PhD thesis, University of Pretoria, Pretoria, viewed yymmdd < http://hdl.handle.net/2263/24273 >
http://upetd.up.ac.za/thesis/available/etd-05012013-153550/
id ndltd-netd.ac.za-oai-union.ndltd.org-up-oai-repository.up.ac.za-2263-24273
record_format oai_dc
collection NDLTD
sources NDLTD
topic Albumin production
Enhanced cell function
Three-dimensional cell culture
Drug metabolism
UCTD
spellingShingle Albumin production
Enhanced cell function
Three-dimensional cell culture
Drug metabolism
UCTD
Rossouw, C.L. (Claire Louise)
Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
description Although conventional two-dimensional (2D) cell culture is convenient for routine work, researchers are turning to three-dimensional (3D) cell culture for more accurate, physiologically representative information on the way their cells behave and respond to stimuli. Cells can now be routinely cultured in the many commercially available 3D formats. In this study, we developed non-woven scaffolds for 3D cell culture and enhanced cell function. By making use of methods that measure the behaviour of liver cells in the 3D system we were able to demonstrate, compared to standard 2D systems, significantly higher expression of key liver enzymes involved in drug metabolism and albumin production (specifically cytochrome P450). Cell proliferation on the various scaffolds was comparable to that of a commercially available hydrogel 3D cell culture system, AlgimatrixTM. When culturing cells in 3D, the means by which cells are harvested or extracted from the 3D scaffold for downstream applications is more challenging than in 2D. For this reason, many of the 3D scaffolds currently manufactured are either bio-degradable or require the use of salts to dissolve the scaffold which may negatively impact on the cells they contain. By grafting the non-woven scaffolds with the thermoresponsive polymer, poly(N-isopropylacrylamide) (PNIPAAm), we demonstrated that cells growing on the scaffolds are able to be released from the scaffold in a 3D conformation, non-enzymatically, through temperature changes. Selected thermoresponsive non-woven fabrics were also tested in an automated cell culture device for cell proliferation and thermally induced harvesting. One of the applications of a 3D cell culturing system would be in exploration of the many diseases plaguing mankind, in particular malaria which is still responsible for severe disease and mortality, especially in Africa. Most available antimalarials are designed to target the pathogenic blood stages in humans and to address the constant threat of drug resistance. However, to meet the objective of malaria eradication, medicines that block parasite transmission also need to be developed. Molecules that efficiently target the parasite stages in the liver would prevent pathogenesis, symptoms and transmission. Equipped with the knowledge that the infectious sporozoites traverse several hepatocytes prior to cell infection, it may be physiologically limiting to culture the exo-erythrocytic stage in vitro in a 2D cell culture system where the hepatocytes are in an unnatural flat conformation, distinctly different to their in vivo counterparts. Moreover, monolayer cell cultures lose their tissue-related functions rapidly, greatly impairing the predictive power of such assays. Thus, the second aim of this thesis was to establish if hepatocytes that have been cultured on 3D non-woven scaffolds improve in vitro sporozoite invasion compared to conventional 2D systems. Sporozoite invasion was detected in the conventional 2D monolayers using a TaqMan® assay but not in the hepatocytes growing in 3D. Future studies beyond the scope of this thesis will include modifications to the 3D scaffold to attempt achieving superior sporozoite invasion in this model system. === Thesis (PhD)--University of Pretoria, 2013. === Biochemistry === unrestricted
author2 Moolman, Samantha
author_facet Moolman, Samantha
Rossouw, C.L. (Claire Louise)
author Rossouw, C.L. (Claire Louise)
author_sort Rossouw, C.L. (Claire Louise)
title Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
title_short Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
title_full Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
title_fullStr Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
title_full_unstemmed Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
title_sort development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture
publishDate 2013
url http://hdl.handle.net/2263/24273
Rossouw, CL 2013, Development and applications of a novel, hermoresponsive scaffold for three-dimensional cell culture, PhD thesis, University of Pretoria, Pretoria, viewed yymmdd < http://hdl.handle.net/2263/24273 >
http://upetd.up.ac.za/thesis/available/etd-05012013-153550/
work_keys_str_mv AT rossouwclclairelouise developmentandapplicationsofanovelthermoresponsivescaffoldforthreedimensionalcellculture
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spelling ndltd-netd.ac.za-oai-union.ndltd.org-up-oai-repository.up.ac.za-2263-242732017-07-20T04:10:33Z Development and applications of a novel, thermoresponsive scaffold for three-dimensional cell culture Rossouw, C.L. (Claire Louise) Moolman, Samantha Birkholtz, Lyn-Marie Mancama, Dalu Hoppe, Heinrich C. clairerossouw@gmail.com Albumin production Enhanced cell function Three-dimensional cell culture Drug metabolism UCTD Although conventional two-dimensional (2D) cell culture is convenient for routine work, researchers are turning to three-dimensional (3D) cell culture for more accurate, physiologically representative information on the way their cells behave and respond to stimuli. Cells can now be routinely cultured in the many commercially available 3D formats. In this study, we developed non-woven scaffolds for 3D cell culture and enhanced cell function. By making use of methods that measure the behaviour of liver cells in the 3D system we were able to demonstrate, compared to standard 2D systems, significantly higher expression of key liver enzymes involved in drug metabolism and albumin production (specifically cytochrome P450). Cell proliferation on the various scaffolds was comparable to that of a commercially available hydrogel 3D cell culture system, AlgimatrixTM. When culturing cells in 3D, the means by which cells are harvested or extracted from the 3D scaffold for downstream applications is more challenging than in 2D. For this reason, many of the 3D scaffolds currently manufactured are either bio-degradable or require the use of salts to dissolve the scaffold which may negatively impact on the cells they contain. By grafting the non-woven scaffolds with the thermoresponsive polymer, poly(N-isopropylacrylamide) (PNIPAAm), we demonstrated that cells growing on the scaffolds are able to be released from the scaffold in a 3D conformation, non-enzymatically, through temperature changes. Selected thermoresponsive non-woven fabrics were also tested in an automated cell culture device for cell proliferation and thermally induced harvesting. One of the applications of a 3D cell culturing system would be in exploration of the many diseases plaguing mankind, in particular malaria which is still responsible for severe disease and mortality, especially in Africa. Most available antimalarials are designed to target the pathogenic blood stages in humans and to address the constant threat of drug resistance. However, to meet the objective of malaria eradication, medicines that block parasite transmission also need to be developed. Molecules that efficiently target the parasite stages in the liver would prevent pathogenesis, symptoms and transmission. Equipped with the knowledge that the infectious sporozoites traverse several hepatocytes prior to cell infection, it may be physiologically limiting to culture the exo-erythrocytic stage in vitro in a 2D cell culture system where the hepatocytes are in an unnatural flat conformation, distinctly different to their in vivo counterparts. Moreover, monolayer cell cultures lose their tissue-related functions rapidly, greatly impairing the predictive power of such assays. Thus, the second aim of this thesis was to establish if hepatocytes that have been cultured on 3D non-woven scaffolds improve in vitro sporozoite invasion compared to conventional 2D systems. Sporozoite invasion was detected in the conventional 2D monolayers using a TaqMan® assay but not in the hepatocytes growing in 3D. Future studies beyond the scope of this thesis will include modifications to the 3D scaffold to attempt achieving superior sporozoite invasion in this model system. Thesis (PhD)--University of Pretoria, 2013. Biochemistry unrestricted 2013-09-06T17:01:23Z 2013-05-17 2013-09-06T17:01:23Z 2013-04-12 2013-05-17 2013-05-01 Thesis http://hdl.handle.net/2263/24273 Rossouw, CL 2013, Development and applications of a novel, hermoresponsive scaffold for three-dimensional cell culture, PhD thesis, University of Pretoria, Pretoria, viewed yymmdd < http://hdl.handle.net/2263/24273 > D13/4/489/ag http://upetd.up.ac.za/thesis/available/etd-05012013-153550/ © 2013 University of Pretoria. All rights reserved. The copyright in this work vests in the University of Pretoria. No part of this work may be reproduced or transmitted in any form or by any means, without the prior written permission of the University of Pretoria.