Silk film biomaterials for cornea tissue engineering

Lawrence, Brian D.; Marchant, Jeffrey K.; Pindrus, Mariya A.; Omenetto, Fiorenzo G.; Kaplan, David L.

doi:10.1016/j.biomaterials.2008.11.018

Cited by 375 publications

(344 citation statements)

References 49 publications

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“…Therefore, in numerous tissue engineering studies, fluorescence microscopy has been used to distinguish matrix and matrix-embedded cells and examine their functionality. [79][80][81] In comparison to conventional optical microscopy, two-or multiphoton fluorescence microscopy can reduce optical attenuation and background signals by multiphoton absorption so that depth-resolved validation of the FIG. 7.…”

Section: Optical Imagingmentioning

confidence: 99%

Imaging Strategies for Tissue Engineering Applications

Nam

Ricles

Suggs

et al. 2015

Tissue Engineering Part B: Reviews

125

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Section: Optical Imagingmentioning

confidence: 99%

Imaging Strategies for Tissue Engineering Applications

Nam

Ricles

Suggs

et al. 2015

Tissue Engineering Part B: Reviews

125

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“…The culture system methodology presented here represents a scalable approach for rapid assessments of cell-silk film surface interactions. Of particular interest is the use of surface patterned silk films to study differences in cell proliferation and responses of cells for alignment 12,14 . The seeded cultures were cultured on both micro-patterned and flat silk film substrates, and then assessed through time-lapse phase-contrast imaging, scanning electron microscopy, and biochemical assessment of metabolic activity and nucleic acid content.…”

mentioning

confidence: 99%

Silk Film Culture System for <em>in vitro</em> Analysis and Biomaterial Design

Lawrence

Pan

Weber

et al. 2012

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Silk films are promising protein-based biomaterials that can be fabricated with high fidelity and economically within a research laboratory environment 1,2 . These materials are desirable because they possess highly controllable dimensional and material characteristics, are biocompatible and promote cell adhesion, can be modified through topographic patterning or by chemically altering the surface, and can be used as a depot for biologically active molecules for drug delivery related applications [3][4][5][6][7][8] . In addition, silk films are relatively straightforward to custom design, can be designed to dissolve within minutes or degrade over years in vitro or in vivo, and are produce with the added benefit of being transparent in nature and therefore highly suitable for imaging applications [9][10][11][12][13] . The culture system methodology presented here represents a scalable approach for rapid assessments of cell-silk film surface interactions. Of particular interest is the use of surface patterned silk films to study differences in cell proliferation and responses of cells for alignment 12,14 . The seeded cultures were cultured on both micro-patterned and flat silk film substrates, and then assessed through time-lapse phase-contrast imaging, scanning electron microscopy, and biochemical assessment of metabolic activity and nucleic acid content. In summary, the silk film in vitro culture system offers a customizable experimental setup suitable to the study of cell-surface interactions on a biomaterial substrate, which can then be optimized and then translated to in vivo models. Observations using the culture system presented here are currently being used to aid in applications ranging from basic cell interactions to medical device design, and thus are relevant to a broad range of biomedical fields. Video LinkThe video component of this article can be found at https://www.jove.com/video/3646/ Protocol Fabrication of Silicone Rubber Molds1. Produce or purchase a desired topographic surface for casting. For this publication a standard 100 mm etched silicon wafer will be described (Figure 1). 2. Weigh out polydimethylsiloxane (PDMS) potting (component A) and catalyst (component B) solution in a 1:9 ratio (9 g potting and 1 g catalyst) as provided in the purchased kit. 3. Mix solutions thoroughly to initiate curing process. 4. Place silicon wafer surface within a casting dish. 5. Weigh out 4.5 g of PDMS solution onto silicon wafer. 6. Spread PDMS solution as to cover a 100 mm diameter area of the wafer surface. 7. Tilt wafer to spread PDMS solution evenly. 8. Cover wafer with 100 mm diameter petri dish lid. 9. Place casting setup into 60 °C oven over night, making certain that curing is taking place on a flat surface. 10. Place cured PDMS/silicon wafer into 70% ethanol bath before removal. 11. Begin removing PDMS from wafer by using razor blade to lift edge (entire circumference) first. 12. Gently pull PDMS off using forceps within a 70% ethanol bath being careful not to tear silicone rubber casting....

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“…Therefore, engineering corneal stroma has been actively investigated by developing functional corneal stroma substrates through chemical, morphological, and mechanical cues. [50][51][52][53][54][55][56][57] In particular, synthetic polymers have been explored for stromal corneal substrates because of their tunable mechanical properties. They have also been processed in micron-nanosized fiber forms to direct stromal cell organization and differentiation in vitro, resulting in stratified collagen fibril lamellae in orthogonal orientations.…”

Section: Corneal Stromamentioning

confidence: 99%

“…Primary human corneal fibroblast cells Torbet et al, 52 Crabb et al, 55 Wilson et al, 56 Gil et al, 65 Lawrence et al, 50 and Reichl et al…”

mentioning

confidence: 99%