Light-activated hydrogel formation via the triggered folding and self-assembly of a designed peptide

被引:0
|
作者
Haines, Lisa A. [1 ]
Rajagopal, Karthikan [1 ]
Ozbas, Bulent [2 ]
Salick, Daphne A. [1 ]
Pochan, Darrin J. [2 ]
Schneider, Joel P. [1 ]
机构
[1] Department of Chemistry and Biochemistry, Delaware Biotechnology Institute, University of Delaware, Newark, DE 19716-2522, United States
[2] Materials Science and Engineering, Delaware Biotechnology Institute, University of Delaware, Newark, DE 19716-2522, United States
来源
Journal of the American Chemical Society | 2005年 / 127卷 / 48期
关键词
Assays - Photopolymerization - Proteins - Reaction kinetics - Self assembly - Spectroscopic analysis;
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学科分类号
摘要
Photopolymerization can be used to construct materials with precise temporal and spatial resolution. Applications such as tissue engineering, drug delivery, the fabrication of microfluidic devices and the preparation of high-density cell arrays employ hydrogel materials that are often prepared by this technique. Current photopolymerization strategies used to prepare hydrogels employ photoinitiators, many of which are cytotoxic and require large macromolecular precursors that need to be functionalized with moieties capable of undergoing radical cross-linking reactions. We have developed a simple light-activated hydrogelation system that employs a designed peptide whose ability to self-assemble into hydrogel material is dependent on its intramolecular folded conformational state. An iterative design strategy afforded MAX7CNB, a photocaged peptide that, when dissolved in aqueous medium, remains unfolded and unable to self-assemble; a 2 wt % solution of freely soluble unfolded peptide is stable to ambient light and has the viscosity of water. Irradiation of the solution (260 < λ < 360 nm) releases the photocage and triggers peptide folding to produce amphiphilic β-hairpins that self-assemble into viscoelastic hydrogel material. Circular dichroic (CD) spectroscopy supports this folding and self-assembly mechanism, and oscillatory rheology shows that the resulting hydrogel is mechanically rigid (G′ = 1000 Pa). Laser scanning confocal microscopy imaging of NIH 3T3 fibroblasts seeded onto the gel indicates that the gel surface is noncytotoxic, conducive to cell adhesion, and allows cell migration. Lastly, thymidine incorporation assays show that cells seeded onto decaged hydrogel proliferate at a rate equivalent to cells seeded onto a tissue culture-treated polystyrene control surface. © 2005 American Chemical Society.
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页码:17025 / 17029
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