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  2. Laboratory exploration of the use of ripasudil in descemetorhexis with a human ex vivo model

Laboratory exploration of the use of ripasudil in descemetorhexis with a human ex vivo model

  • Exp Eye Res. 2024 Jun 18:245:109977. doi: 10.1016/j.exer.2024.109977.
Meidong Zhu 1 Li Wen 1 Barbara Burgos-Blasco 2 Luke C Northey 3 Natasha Spiteri 4 Constantinos Petsoglou 3 Gregory Moloney 3
Affiliations

Affiliations

  • 1 New South Wales Tissue Bank, New South Wales Organ and Tissue Donation Service, Sydney, Australia; The University of Sydney, Sydney, Australia.
  • 2 University of British Columbia, Vancouver, Canada. Electronic address: bburgos171@hotmail.com.
  • 3 The University of Sydney, Sydney, Australia; Sydney Eye Hospital, Sydney, Australia.
  • 4 Ophthalmology, Countess of Chester Hospital, Chester, United Kingdom; Newmedica, Shrewsbury, United Kingdom.
Abstract

The aim of the study was to investigate the effect of ripasudil on corneal endothelial cell survival and migration after two types of descemetorhexis on a human ex vivo model. Eleven human corneoscleral buttons were incubated in either 50 ml organ culture medium containing 10 μM ripasudil or 50 μl dimethyl sulfoxide (DMSO), the vehicle in ripasudil for 2 days prior to wound creation then for 14 days after. The wound was created with either full trephination scoring or by shallow trephination plus manual peeling. At day 14, immunohistochemistry with vimentin and Na+/K+/ATPase markers was conducted. Tissues were assessed at day 3, 7 and 14 for morphology, cell migration, cell viability and cell density. Full trephination scoring created more damage on tissues compared to shallow trephination with full Descemet membrane peeling. In the full trephination scoring group, no differences in cell viability were noted when ripasudil and DMSO were compared. With the peeling method, Ripasudil could protect the endothelial cell death and maintain the morphology compared to the control. At day 14, no differences in the peripheral cell viability and density were found between ripasudil and DMSO, although the ripasudil group presented significantly increased central cell count and cell viability. Increased cell migration was noted with ripasudil and the initial cell morphology of those migrated cells was similar to that of fibroblasts. In conclusion, ex vivo modelling suggested that peeling resulted in less cell damage than scoring and ripasudil maintained better morphology and promoted migration. These effects might be via transformation of endothelial cells into a more motile spindle-like phenotype.

Keywords

Descemet membrane; Fuchs endothelial corneal dystrophy; Ripasudil.

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