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Please use this identifier to cite or link to this item: http://hdl.handle.net/11375/22743
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dc.contributor.advisorWylie, Ryan G.-
dc.contributor.authorNijsure, Devang-
dc.date.accessioned2018-04-23T16:44:01Z-
dc.date.available2018-04-23T16:44:01Z-
dc.date.issued2018-
dc.identifier.urihttp://hdl.handle.net/11375/22743-
dc.description.abstractThe in vivo 3D extracellular matrix provides a temporal regulatory environment of chemical cues. Understanding this dynamic environment will be crucial for efficient drug screening, diseases mechanism elucidation, and tissue engineering. Therefore, in vitro 3D cell culture systems with reversible chemical environments are required. To this end, we developed a non-cytotoxic agarose-desthiobiotin hydrogel to sequester streptavidin biomolecule conjugates (KD 10-11 M), which can then be displaced by the addition of biotin (KD 10-15 M). Streptavidin biomolecule conjugates were simultaneously and sequentially immobilized by changing media components. The time required for biochemical environment exchange was minimized by increasing the surface area to volume ratios and pore size of the hydrogels. We temporally controlled the cell adhesive properties of hydrogels with RGD modified streptavidin to influence endothelial cell tube formation.en_US
dc.language.isoenen_US
dc.subjectHydrogelsen_US
dc.subjectBiomaterialen_US
dc.subjectTissue Engineeringen_US
dc.subject3D Cell Cultureen_US
dc.subjectDynamicen_US
dc.subjectExtracellular Matrixen_US
dc.titleHydrogels with Dynamic Biochemical Environment for 3D Cell Cultureen_US
dc.typeThesisen_US
dc.contributor.departmentChemical Biologyen_US
dc.description.degreetypeThesisen_US
dc.description.degreeMaster of Science (MSc)en_US
Appears in Collections:Open Access Dissertations and Theses

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