High-throughput studies of cells mechanotransduction are usually performed using 2D biomaterials. However, cells-extracellular matrix interactions in the body occur in 3D environment. By using cells entrapped in hydrogels, it is not easy to isolate the mechanical effect from the chemical cues of biomaterials. We used a cytocompatible and non-expensive platform based in the patterning of wettable spots in superhydrophobic surfaces to deposit porous biomaterials in these regions. Freeze-dried alginate/chitosan scaffolds were used to create an array of mechanical properties and porosities. Adaptation of dynamic mechanic analysis equipment allowed performing on-chip single scaffold analysis. Micro-computed tomography allowed acquir- ing data for whole chips simultaneously. Results were validated using individual scaffolds and single-formulation chips. A sub-array with combined modulus/porosity properties was selected. Fibronectin (Fn) in different concentration was adsorbed in the scaffolds, and fibroblasts and osteoblast-like cells were seeded. The independent study of variables influence in cell response was performed by image-based methods. In the absence of Fn fibroblasts did not respond to mechani- cal properties in the chip range. Osteoblast-like cells showed higher cell adhesion in stiffer substrates. The adsorption of Fn was studied qualita- tively by image methods. Results related with Fn amount and scaffolds’ mechanical properties were analyzed for each cell type.</p

Mano, J. F.

Oliveira, Mariana B.

Salgado, Christiane L.

Journal of Tissue Engineering and Regenerative Medicine

Universidade do Minho: RepositoriUM

37.P07
Superhydrophobic platforms for the
combinatorial analysis of biomaterials-cells
interactions using arrays of 3D scaffolds with
distinct mechanical and morphological properties
MB Oliveira, CL Salgado and JF Mano
3B’s Research Group–Biomaterials, Biodegradables &
Biomimetics, Univ. of Minho, Headquarters of the European
Institute of Excellence on Tiss. Eng.&Regen. Med., ICVS/3B’s-PT
Government Assoc. Laboratory, Portugal
High-throughput studies of cells mechanotransduction are usually
performed using 2D biomaterials. However, cells-extracellular matrix
interactions in the body occur in 3D environment. By using cells
entrapped in hydrogels, it is not easy to isolate the mechanical effect
from the chemical cues of biomaterials. We used a cytocompatible and
non-expensive platform based in the patterning of wettable spots in
superhydrophobic surfaces to deposit porous biomaterials in these
regions. Freeze-dried alginate/chitosan scaffolds were used to create
an array of mechanical properties and porosities. Adaptation of
dynamic mechanic analysis equipment allowed performing on-chip
single scaffold analysis. Micro-computed tomography allowed acquir-
ing data for whole chips simultaneously. Results were validated using
individual scaffolds and single-formulation chips. A sub-array with
combined modulus/porosity properties was selected. Fibronectin (Fn)
in different concentration was adsorbed in the scaffolds, and fibroblasts
and osteoblast-like cells were seeded. The independent study of
variables influence in cell response was performed by image-based
methods. In the absence of Fn fibroblasts did not respond to mechani-
cal properties in the chip range. Osteoblast-like cells showed higher cell
adhesion in stiffer substrates. The adsorption of Fn was studied qualita-
tively by image methods. Results related with Fn amount and scaffolds’
mechanical properties were analyzed for each cell type.
37.P08
Extrinsic biophysical stimulus can override the
influence of local substrate in determining stem
cell fate
SD Thorpe, CT Buckley, AJ Steward, DJ Kelly
Trinity Centre for Bioengineering, Trinity College Dublin, Ireland;
Department of Mechanical Engineering, University of Notre
Dame, Ireland
The aim of this study was to explore how cell-matrix interactions and
extrinsic mechanical signals interact to determine stem cell fate in
response to transforming growth factor-b3 (TGF-b3). Bone marrow
derived mesenchymal stem cells (MSCs) were seeded in agarose and
fibrin hydrogels and subjected to dynamic compression in the presence
of TGF-b3. Markers of chondrogenic, myogenic and endochondral dif-
ferentiation were assessed. Free-swelling agarose constructs stained
positively for chondrogenic markers, and appeared to be progressing
towards terminal differentiation as indicated by collagen type X and
mineral staining. Dynamic compression suppressed differentiation
along this endochondral pathway. In contrast, fibrin constructs sup-
ported differentiation along an alternative myogenic pathway in long-
term free-swelling culture. Given that fibrin clots support a chondro-
genic phenotype in vivo within mechanically loaded joint defect envi-
ronments, the influence of long term dynamic compression on MSC
differentiation was investigated. Mechanical signals generated by this
extrinsic loading ultimately governed MSC fate, directing MSCs along
a chondrogenic pathway as opposed to the default myogenic pheno-
type supported within unloaded fibrin clots. In conclusion, this study
demonstrates that external cues such as the mechanical environment
can override the influence of specific substrates, scaffolds or hydrogels
on determining mesenchymal stem cell fate.
37.P09
Evaluation of cell response on permanent and
pulsed atmospheric pressure stressed cells
B Rieder, AWeihs, A Teuschl, G Knebl, J Kollmitzer, H Redl
and D Rünzler
University of Applied Sciences Technikum Wien, Austria; Ludwig
Boltzmann Institute for Experimental and Clinical Traumatology,
TGM - Die Schule der Technik, Austria
Introduction: Many studies display that mechanical stimuli already ful-
fill the needs for cell differentiation, without any need for additional
growth factors. Thus, we concentrated on mechanical stimuli of atmo-
spheric pressure on cells using a tailor-made pressure chamber. Aim of
the study was to determine pressure limits of cells and possible side
effects to find supporting conditions for cell proliferation or differentia-
tion.
Materials and methods: Cells of the cell lines U937 and MG63 were per-
manently kept at 37C and buffered with HEPES during the experi-
ments. The atmospheric pressure was applied on 1- respectively 2-well-
chamberslides in the pressure chamber. For static pressure experiments,
cells were permanently stimulated at 200, 300 or 400 kPa for 1 respec-
tively 12 h and cultured for 2 weeks afterwards. For dynamic pressure
experiments, pressures between 300 and 400 kPa were applied at fre-
quencies of 0.25–4 Hz. Cell growth was observed for 5 days and evalu-
ated by trypan blue staining and MTTassay.
Results: We could not observe any negative or positive effects on cell
proliferation after the static pressure mode experiments. In the dynami-
cal pressure experiment, 24 h after last pressure exposure, cells
restored the original conditions and gave the same read-out compared
to the untreated control.
Discussion: Thus, our tailor-made pressure chamber seems to be appro-
priate to find more specific parameters that induce cell differentiation
of adult stem cells.
37.P10
Epigenetic modification of beta-catenin in 3D
Titania mesenchymal cell cultured scaffolds
under variable flux conditions in bioreactor
chambers
R Couceiro, A Gil, C Garcia, P Diaz, J Couceiro, M Freire-Garabal
and F Guitian
Institute of Ceramcis, USC, Spain; School Of Medicin, Dept of
Pharmacolog, USC, Spain; School of Pharmacy, USC, Spain;
Royal Academy of Medicine, Spain
Mesenchymal stem cell fate determination is heavily regulated by the
WNT pathway through b-Catenin.Biomaterial topography triggers cyto-
skeleton biochemical and physical responses, which will ultimately
modify gene expression leading to an osteoblastic phenotype. It is
already known that several cytoskeleton related genes are mechanoreg-
ulated. In this study as a result of exploring epigenetic regulations by
methylation levels of Beta-Catenin, a more accurate insight of osteo-
genic control could be achieved. Engineering a stem cell niche is a task
that considers not just a 3D scaffold which will mimic a cellular micro-
environment, but also the dynamic forces exerted on cultured stem
cells.A functional tissue engineering (FTE) method could be completed
by identifying methylation patterns within dynamic culture mod-
els.Titania (TiO2) scaffolds were synthesized with pore sizes ranging
from 300–400 lm by Direct Ink Writing and cultured with human mes-
enchymal stem cells. In order to evaluate the existence of potential dif-
ferential methylation rates, scaffolds were placed in a bioreactor
chamber under pulsed flux conditions (2, 6, and 12 h). A non flux con-
trol group was used. Methylation specific polymerase chain reaction
(MSP) and direct sequencing showed how CpG islands related to Beta
Catenin are being directly modified under variable flux conditions
 2012 The Authors J Tissue Eng Regen Med 2012; 6 (Suppl. 1): 1–429.
Journal of Tissue Engineering and Regenerative Medicine 2012 John Wiley & Sons, Ltd. DOI: 10.1002/term.1586
240 37. Mechanotransduction in TERM


English

Superhydrophobic platforms for the combinatorial analysis of biomaterials-cells interactions using arrays of 3D scaffolds with distinct mechanical and morphological properties

37.P07Superhydrophobic platforms for thecombinatorial analysis of biomaterials-cellsinteractions using arrays of 3D scaffolds withdistinct mechanical and morphological propertiesMB Oliveira, CL Salgado and JF Mano3B’s Research Group–Biomaterials, Biodegradables &Biomimetics, Univ. of Minho, Headquarters of the EuropeanInstitute of Excellence on Tiss. Eng.&Regen. Med., ICVS/3B’s-PTGovernment Assoc. Laboratory, PortugalHigh-throughput studies of cells mechanotransduction are usuallyperformed using 2D biomaterials. However, cells-extracellular matrixinteractions in the body occur in 3D environment. By using cellsentrapped in hydrogels, it is not easy to isolate the mechanical effectfrom the chemical cues of biomaterials. We used a cytocompatible andnon-expensive platform based in the patterning of wettable spots insuperhydrophobic surfaces to deposit porous biomaterials in theseregions. Freeze-dried alginate/chitosan scaffolds were used to createan array of mechanical properties and porosities. Adaptation ofdynamic mechanic analysis equipment allowed performing on-chipsingle scaffold analysis. Micro-computed tomography allowed acquir-ing data for whole chips simultaneously. Results were validated usingindividual scaffolds and single-formulation chips. A sub-array withcombined modulus/porosity properties was selected. Fibronectin (Fn)in different concentration was adsorbed in the scaffolds, and fibroblastsand osteoblast-like cells were seeded. The independent study ofvariables influence in cell response was performed by image-basedmethods. In the absence of Fn fibroblasts did not respond to mechani-cal properties in the chip range. Osteoblast-like cells showed higher celladhesion in stiffer substrates. The adsorption of Fn was studied qualita-tively by image methods. Results related with Fn amount and scaffolds’mechanical properties were analyzed for each cell type.37.P08Extrinsic biophysical stimulus can override theinfluence of local substrate in determining stemcell fateSD Thorpe, CT Buckley, AJ Steward, DJ KellyTrinity Centre for Bioengineering, Trinity College Dublin, Ireland;Department of Mechanical Engineering, University of NotreDame, IrelandThe aim of this study was to explore how cell-matrix interactions andextrinsic mechanical signals interact to determine stem cell fate inresponse to transforming growth factor-b3 (TGF-b3). Bone marrowderived mesenchymal stem cells (MSCs) were seeded in agarose andfibrin hydrogels and subjected to dynamic compression in the presenceof TGF-b3. Markers of chondrogenic, myogenic and endochondral dif-ferentiation were assessed. Free-swelling agarose constructs stainedpositively for chondrogenic markers, and appeared to be progressingtowards terminal differentiation as indicated by collagen type X andmineral staining. Dynamic compression suppressed differentiationalong this endochondral pathway. In contrast, fibrin constructs sup-ported differentiation along an alternative myogenic pathway in long-term free-swelling culture. Given that fibrin clots support a chondro-genic phenotype in vivo within mechanically loaded joint defect envi-ronments, the influence of long term dynamic compression on MSCdifferentiation was investigated. Mechanical signals generated by thisextrinsic loading ultimately governed MSC fate, directing MSCs alonga chondrogenic pathway as opposed to the default myogenic pheno-type supported within unloaded fibrin clots. In conclusion, this studydemonstrates that external cues such as the mechanical environmentcan override the influence of specific substrates, scaffolds or hydrogelson determining mesenchymal stem cell fate.37.P09Evaluation of cell response on permanent andpulsed atmospheric pressure stressed cellsB Rieder, AWeihs, A Teuschl, G Knebl, J Kollmitzer, H Redland D Ru¨nzlerUniversity of Applied Sciences Technikum Wien, Austria; LudwigBoltzmann Institute for Experimental and Clinical Traumatology,TGM - Die Schule der Technik, AustriaIntroduction: Many studies display that mechanical stimuli already ful-fill the needs for cell differentiation, without any need for additionalgrowth factors. Thus, we concentrated on mechanical stimuli of atmo-spheric pressure on cells using a tailor-made pressure chamber. Aim ofthe study was to determine pressure limits of cells and possible sideeffects to find supporting conditions for cell proliferation or differentia-tion.Materials and methods: Cells of the cell lines U937 and MG63 were per-manently kept at 37C and buffered with HEPES during the experi-ments. The atmospheric pressure was applied on 1- respectively 2-well-chamberslides in the pressure chamber. For static pressure experiments,cells were permanently stimulated at 200, 300 or 400 kPa for 1 respec-tively 12 h and cultured for 2 weeks afterwards. For dynamic pressureexperiments, pressures between 300 and 400 kPa were applied at fre-quencies of 0.25–4 Hz. Cell growth was observed for 5 days and evalu-ated by trypan blue staining and MTTassay.Results: We could not observe any negative or positive effects on cellproliferation after the static pressure mode experiments. In the dynami-cal pressure experiment, 24 h after last pressure exposure, cellsrestored the original conditions and gave the same read-out comparedto the untreated control.Discussion: Thus, our tailor-made pressure chamber seems to be appro-priate to find more specific parameters that induce cell differentiationof adult stem cells.37.P10Epigenetic modification of beta-catenin in 3DTitania mesenchymal cell cultured scaffoldsunder variable flux conditions in bioreactorchambersR Couceiro, A Gil, C Garcia, P Diaz, J Couceiro, M Freire-Garabaland F GuitianInstitute of Ceramcis, USC, Spain; School Of Medicin, Dept ofPharmacolog, USC, Spain; School of Pharmacy, USC, Spain;Royal Academy of Medicine, SpainMesenchymal stem cell fate determination is heavily regulated by theWNT pathway through b-Catenin.Biomaterial topography triggers cyto-skeleton biochemical and physical responses, which will ultimatelymodify gene expression leading to an osteoblastic phenotype. It isalready known that several cytoskeleton related genes are mechanoreg-ulated. In this study as a result of exploring epigenetic regulations bymethylation levels of Beta-Catenin, a more accurate insight of osteo-genic control could be achieved. Engineering a stem cell niche is a taskthat considers not just a 3D scaffold which will mimic a cellular micro-environment, but also the dynamic forces exerted on cultured stemcells.A functional tissue engineering (FTE) method could be completedby identifying methylation patterns within dynamic culture mod-els.Titania (TiO2) scaffolds were synthesized with pore sizes rangingfrom 300–400 lm by Direct Ink Writing and cultured with human mes-enchymal stem cells. In order to evaluate the existence of potential dif-ferential methylation rates, scaffolds were placed in a bioreactorchamber under pulsed flux conditions (2, 6, and 12 h). A non flux con-trol group was used. Methylation specific polymerase chain reaction(MSP) and direct sequencing showed how CpG islands related to BetaCatenin are being directly modified under variable flux conditions 2012 The Authors J Tissue Eng Regen Med 2012; 6 (Suppl. 1): 1–429.Journal of Tissue Engineering and Regenerative Medicine 2012 John Wiley & Sons, Ltd. DOI: 10.1002/term.1586240 37. Mechanotransduction in TERM

http://repositorium.sdum.uminho.pt/bitstream/1822/23151/1/termis2012_2.pdf

Superhydrophobic platforms for the combinatorial analysis of biomaterials-cells interactions using arrays of 3D scaffolds with distinct mechanical and morphological properties

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