The effect of Rho Kinase inhibition on corneal nerve regeneration in vitro and in vivo

被引:9
|
作者
Mertsch, Sonja [1 ]
Neumann, Inga [2 ]
Rose, Cosima [2 ]
Schargus, Marc [2 ,3 ]
Geerling, Gerd [2 ]
Schrader, Stefan [1 ]
机构
[1] Carl von Ossietzky Univ Oldenburg, Pius Hosp, Dept Ophthalmol, Lab Expt Ophthalmol, Carl von Ossietzky Str 9-11, D-26129 Oldenburg, Germany
[2] Heinrich Heine Univ, Univ Hosp Duesseldorf, Dept Ophthalmol, Lab Expt Ophthalmol, Dusseldorf, Germany
[3] Asklepios Hosp Nord Heidberg, Dept Ophthalmol, Hamburg, Germany
来源
OCULAR SURFACE | 2021年 / 22卷
关键词
3D model; Corneal nerve regeneration; Cornea; Neurotrophic keratopathy; Rho kinase inhibitor; PLASTIC COMPRESSED COLLAGEN; GROWTH-FACTOR; PENETRATING KERATOPLASTY; CONFOCAL MICROSCOPY; NEURONS; ACTIN; TRANSPLANTATION; REINNERVATION; NEUROPATHY; SUBSTRATE;
D O I
10.1016/j.jtos.2021.08.011
中图分类号
R77 [眼科学];
学科分类号
100212 ;
摘要
Purpose: Impairment of corneal nerves can lead to neurotrophic keratopathy accompanied with severe ocular surface damage, which due to limited treatment options, can result in severe visual deterioration. This study evaluates a possible new treatment by enhancing the corneal nerve regeneration using a Rho Kinase inhibitor (Y27632). ROCK is known to play an important role in regulating cell morphology, adhesion and motility but little is known about its role in corneal nerve regeneration. Methods: Effects of ROCK inhibition on murine peripheral nerves was assessed in single cell-and wound healing assays as well as a 3D in vitro model. Furthermore, Sholl analysis evaluating neuronal branching and life-death assays evaluating toxicity of the inhibitor were performed. An in vivo mouse model was established, with monitoring weekly corneal nerve regrowth using confocal microscopy. Additionally, corneal nerve fiber length was evaluated by immunofluorescence staining. Underlying pathways were examined by qrtPCR. Results: ROCK inhibition leads to a significant enhancement of fiber growth in vitro. Sholl analysis revealed a higher degree of branching of treated fibers. Cytotoxicity assay showed no influence of Y27632 on cellular survival. In vivo measurement revealed significant enhanced regeneration after injury in the treated group. QrtPCR of trigeminal ganglia confirmed ROCK knock-down as well as altered pathways. Conclusion: The inhibition of ROCK after corneal nerve injury resulted in an enhanced regrowth of fibers in vitro and in vivo. This might be a step towards a new therapeutic concept for the treatment of impaired corneal nerves in diseases such as neurotrophic keratopathy.
引用
收藏
页码:213 / 223
页数:11
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