4.5 Article

Long-Term Study of Corneal Stroma and Endothelium on Structure and Cells After Genipin Treatment of Rabbit Corneas

Journal

Publisher

ASSOC RESEARCH VISION OPHTHALMOLOGY INC
DOI: 10.1167/tvst.10.5.9

Keywords

genipin; crosslinking; keratocytes; endothelium

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Funding

  1. Beijing Natural Science Foundation [7192210]
  2. Scientific Research Seed Fund of Peking University First Hospital [2020SF07]
  3. National Natural Science Foundation of China [11372011]

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The study found that local genipin immersion crosslinking without corneal epithelium can activate keratocytes in the corneal stroma and is relatively safe for thin corneas. Genipin not only crosslinks collagen fibers but also activates keratocytes, and may even promote the secretion of collagen fibers.
Purpose: To study the long-term safety of genipin treatment using a vacuum device with or without epithelial cells at different crosslinking times. Methods: Twenty-five healthyNew Zealandwhite rabbitswere separated into five treatment groups: 0.25% genipin with epithelial cells for 5 minutes (G1), 0.25% genipin without epithelial cells for 5 minutes (G2), 0.25% genipin without epithelial cells for 10 minutes (G3), ultraviolet A-riboflavin collagen crosslinking (UVA), and controls (C). Before and 2, 4, 6, and 8 weeks after crosslinking treatment, anterior segment optical coherence tomography (ASOCT), in vivo confocalmicroscopy (IVCM), and the Pentacam system were used to evaluate the right eyes. Results: A demarcation line (DL) was observed in the corneal stroma in the G2, G3, and UVA groups. The DL depths in the G2 and G3 groups were stable but decreased in the UVA group over time. The density of keratocytes in these groups increased. Endothelial cell density was decreased in the UVA group. There were no differences in the endothelium before and after treatment in the G1, G2, G3, and C groups. The densitometry, as determined using the Pentacam system, significantly increased in the G2, G3, and UVA groups and was positively correlated with keratocyte densities. Conclusions: A vacuum ring assisting local genipin immersion crosslinking without corneal epithelium can activate the keratocytes in the corneal stroma and was safe enough for the thin cornea. Translational Relevance: Genipin can not only crosslink the collagen fibers but also activate the keratocytes and even may promote collagen fiber secretion.

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