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Matrix degradability controls multicellularity of 3D cell migration
by
Polacheck, William J.
, Baker, Brendon M.
, Burdick, Jason A.
, Chen, Christopher S.
, Choi, Colin K.
, Trappmann, Britta
in
631/1647/277
/ 631/61/2035
/ 631/61/54
/ 631/80/84/750
/ Angiogenesis
/ Biomedical materials
/ Cell adhesion & migration
/ Cell Movement
/ Cell Proliferation
/ Degradability
/ Endothelial cells
/ Human Umbilical Vein Endothelial Cells - cytology
/ Humanities and Social Sciences
/ Humans
/ Hydrogel, Polyethylene Glycol Dimethacrylate - chemistry
/ Hydrogels
/ Leukocyte migration
/ Material properties
/ Microfluidics
/ Microfluidics - instrumentation
/ multidisciplinary
/ Neovascularization, Physiologic
/ Science
/ Science (multidisciplinary)
/ Switches
/ Tissue engineering
/ Tissue Engineering - instrumentation
2017
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Matrix degradability controls multicellularity of 3D cell migration
by
Polacheck, William J.
, Baker, Brendon M.
, Burdick, Jason A.
, Chen, Christopher S.
, Choi, Colin K.
, Trappmann, Britta
in
631/1647/277
/ 631/61/2035
/ 631/61/54
/ 631/80/84/750
/ Angiogenesis
/ Biomedical materials
/ Cell adhesion & migration
/ Cell Movement
/ Cell Proliferation
/ Degradability
/ Endothelial cells
/ Human Umbilical Vein Endothelial Cells - cytology
/ Humanities and Social Sciences
/ Humans
/ Hydrogel, Polyethylene Glycol Dimethacrylate - chemistry
/ Hydrogels
/ Leukocyte migration
/ Material properties
/ Microfluidics
/ Microfluidics - instrumentation
/ multidisciplinary
/ Neovascularization, Physiologic
/ Science
/ Science (multidisciplinary)
/ Switches
/ Tissue engineering
/ Tissue Engineering - instrumentation
2017
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Matrix degradability controls multicellularity of 3D cell migration
by
Polacheck, William J.
, Baker, Brendon M.
, Burdick, Jason A.
, Chen, Christopher S.
, Choi, Colin K.
, Trappmann, Britta
in
631/1647/277
/ 631/61/2035
/ 631/61/54
/ 631/80/84/750
/ Angiogenesis
/ Biomedical materials
/ Cell adhesion & migration
/ Cell Movement
/ Cell Proliferation
/ Degradability
/ Endothelial cells
/ Human Umbilical Vein Endothelial Cells - cytology
/ Humanities and Social Sciences
/ Humans
/ Hydrogel, Polyethylene Glycol Dimethacrylate - chemistry
/ Hydrogels
/ Leukocyte migration
/ Material properties
/ Microfluidics
/ Microfluidics - instrumentation
/ multidisciplinary
/ Neovascularization, Physiologic
/ Science
/ Science (multidisciplinary)
/ Switches
/ Tissue engineering
/ Tissue Engineering - instrumentation
2017
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Matrix degradability controls multicellularity of 3D cell migration
Journal Article
Matrix degradability controls multicellularity of 3D cell migration
2017
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Overview
A major challenge in tissue engineering is the development of materials that can support angiogenesis, wherein endothelial cells from existing vasculature invade the surrounding matrix to form new vascular structures. To identify material properties that impact angiogenesis, here we have developed an in vitro model whereby molded tubular channels inside a synthetic hydrogel are seeded with endothelial cells and subjected to chemokine gradients within a microfluidic device. To accomplish precision molding of hydrogels and successful integration with microfluidics, we developed a class of hydrogels that could be macromolded and micromolded with high shape and size fidelity by eliminating swelling after polymerization. Using this material, we demonstrate that matrix degradability switches three-dimensional endothelial cell invasion between two distinct modes: single-cell migration and the multicellular, strand-like invasion required for angiogenesis. The ability to incorporate these tunable hydrogels into geometrically constrained settings will enable a wide range of previously inaccessible biomedical applications.
The fabrication of vascularized 3D tissues requires an understanding of how material properties govern endothelial cell invasion into the surrounding matrix. Here the authors integrate a non-swelling synthetic hydrogel with a microfluidic device to study chemokine gradient-driven angiogenic sprouting and find that matrix degradability modulates the collectivity of cell migration.
Publisher
Nature Publishing Group UK,Nature Publishing Group,Nature Portfolio
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