<em>In Vitro</em> and <em>In Vivo</em> Models to Study Corneal Endothelial-mesenchymal Transition

Wei-Ting Ho; Chien-Chia Su; Jung-Shen Chang; Shu-Wen Chang; Fung-Rong Hu; Tzuu-Shuh Jou; I-Jong Wang

doi:10.3791/54329

JoVE Journal > Developmental Biology

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Gelişim Biyolojisi

생체 외 및 생체 내 모델에서 각막 내피 세포 - 중간 엽 전이를 공부하기

Published: August 20, 2016

doi:

10.3791/54329

Wei-Ting Ho^1,2, Chien-Chia Su³, Jung-Shen Chang³, Shu-Wen Chang¹, Fung-Rong Hu³, Tzuu-Shuh Jou^2,4, I-Jong Wang^3,4

¹Department of Ophthalmology,Far Eastern Memorial Hospital, ²Institute of Clinical Medicine,National Taiwan University, ³Department of Ophthalmology,National Taiwan University Hospital, ⁴College of Medicine,National Taiwan University

Özet

소 각막 내피 세포의 일차 배양 각막 내피 간엽 전이의 메커니즘을 조사 하였다. 또한, 래트 각막 내피 cryoinjury 모델 생체 내 각막 내피 간엽 전환을 증명 하였다.

Abstract

Corneal endothelial cells (CECs) play a crucial role in maintaining corneal clarity through active pumping. A reduced CEC count may lead to corneal edema and diminished visual acuity. However, human CECs are prone to compromised proliferative potential. Furthermore, stimulation of cell growth is often complicated by gradual endothelial-mesenchymal transition (EnMT). Therefore, understanding the mechanism of EnMT is necessary for facilitating the regeneration of CECs with competent function. In this study, we prepared a primary culture of bovine CECs by peeling the CECs with Descemet’s membrane from the corneal button and demonstrated that bovine CECs exhibited the EnMT process, including phenotypic change, nuclear translocation of β-catenin, and EMT regulators snail and slug, in the in vitro culture. Furthermore, we used a rat corneal endothelium cryoinjury model to demonstrate the EnMT process in vivo. Collectively, the in vitro primary culture of bovine CECs and in vivo rat corneal endothelium cryoinjury models offers useful platforms for investigating the mechanism of EnMT.

Introduction

Corneal endothelial cells (CECs) play a vital role in maintaining corneal clarity and thus visual acuity by regulating the hydration status of the corneal stroma through active pumping¹. Because of the limited proliferative potential of human CECs, the cell number decreases with age, and the repair of corneal endothelial wounds following injury is usually achieved through cell enlargement and migration, rather than cell mitosis². When the CEC count decreases below a threshold of approximately 500 cells/mm², the dehydration status of the corneal stroma cannot be maintained, leading to bullous keratopathy and vision impairment^3,4.

The limited proliferative potential of human CECs has been attributed to several factors, including reduced expression of the epidermal growth factor and its receptor in aging cells⁵, antiproliferative TGFβ2 in the aqueous humor⁶, and contact inhibition^2,7. Although some growth factors, such as basic fibroblast growth factor (bFGF), can increase proliferation in a cultured human corneal endothelium, the culture efficiency remains limited^8,9. Furthermore, CECs may undergo a phenotypic change during ex vivo expansion, resembling epithelial-mesenchymal transition (EMT)^10-13. Endothelial-mesenchymal transition (EnMT) is characterized by cell junction destabilization, apical-basal polarity loss, cytoskeletal rearrangement, alpha smooth muscle actin expression, and type I collagen secretion¹⁴. All of these characteristics may abrogate the normal function of CECs, hampering the use of ex vivo cultured CECs in tissue engineering. Moreover, EnMT has been associated with the pathogenesis of several corneal endothelial diseases, including Fuchs endothelial corneal dystrophy and retrocorneal membrane formation^15,16. Therefore, understanding the mechanism of EnMT may aid in manipulating the EnMT process and facilitate the regeneration of CECs to enable competent function.

In this study, we described a method for isolating bovine CECs from the corneal button. In the primary culture in vitro, the EnMT process, including a phenotypic change, the nuclear translocation of β-catenin, and EMT regulators snail and slug, was observed. We further described a method for demonstrating EnMT in vivo by using a rat corneal endothelium cryoinjury model. Using these 2 models, we demonstrated that marimastat, a broad-spectrum matrix metalloproteinase (MMP) inhibitor, can suppress the EnMT process. The described protocols facilitate the detailed analysis of the EnMT mechanism and the development of strategies for manipulating the EnMT process for further clinical application.

Protocol

모든 절차는 안과 및 비전 연구에서 동물의 사용을위한 비전 및 안과 문에 연구를위한 협회 부여 본 연구에서 다음과 국립 대만 대학 병원의 기관 동물 관리 및 사용위원회에 의해 승인되었습니다. 1. 격리, 차 문화의 제조 및 소 CECs의 면역 염색 로컬 도살장에서 신선한 소 눈을 획득. 3 분 동안 10 %의 v / w 포비돈 요오드 용액에 눈 소독. 인산염 완충 식염수 (PBS) 솔루션을 씻으…

Representative Results

소 CECs의 분리 후, 세포를 시험관 내에서 배양 하였다. (1)가 소 CECs의 위상차 이미지를 보여주고있다. 합류 셀의 육각형은 세포가 세포 분리 동안 각막의 간질 섬유 아세포에 의해 오염되지 않은 것으로 나타났다. (2)는 지정된 시점에서 ABC, 달팽이와 민달팽이에 대한 항체를 이용하여 수행 한 면역 염색을 보여주고있다.</s…

Discussion

CECs는 세포 증식 동안 EnMT를 받아야하는 그들의 성향 알려져있다. 치료 목적 EnMT 처리를 억제하기위한 전략을 개발하려면 EnMT기구의 완전한 이해가 필요하다. 우리는 EnMT, 체외 배양 모델 쥐의 각막 내피 세포의 cryoinjury 모델, 즉 소 CEC를 조사하기 위해이 모델을 설명했다. 우리의 결과는 두 모델의 EnMT 과정을 보여 주었다. 또한, 타틴의 EnMT 억제 효과는이 두 모델은 동일한 메커니즘을…

Açıklamalar

The authors have nothing to disclose.

Acknowledgements

We thank the staff of the Second Core Lab, Department of Medical Research, National Taiwan University Hospital for their technical support.

Materials

trypsin	ThermoFisher Scientific	12604-013
Dulbecco’s modified Eagle medium and Ham's F12 medium	ThermoFisher Scientific	11330
fetal bovine serum	ThermoFisher Scientific	26140-079
dimethyl sulfoxide	Sigma	D2650
human epidermal growth factor	ThermoFisher Scientific	PHG0311
insulin, transferrin, selenium	ThermoFisher Scientific	41400-045
cholera toxin	Sigma	C8052-1MG
gentamicin	ThermoFisher Scientific	15750-060
amphotericin B	ThermoFisher Scientific	15290-026
paraformaldehyde	Electron Microscopy Sciences	111219
Triton X-100	Sigma	T8787
bovine serum albumin	Sigma	A7906
marimastat	Sigma	M2699-25MG
anti-active beta-catenin antibody	Millpore	05-665
anti-snail antibody	Santa cruz	sc28199
anti-slug antibody	Santa cruz	sc15391
goat anti-mouse IgG (H+L) secondary antibody	ThermoFisher Scientific	A-11001	for staining of ABC of bovine CECs
goat anti-mouse IgG (H+L) secondary antibody	ThermoFisher Scientific	A-11003	for staining of ABC of rat corneal endothelium
goat anti-rabbit IgG (H+L) secondary antibody	ThermoFisher Scientific	A-11008	for staining of snail and slug of bovine CECs
antibody diluent	Genemed Biotechnologies	10-0001
4',6-diamidino-2-phenylindole	ThermoFisher Scientific	D1306
mounting medium	Vector Laboratories	H-1000
laser scanning confocal microscope	ZEISS	LSM510
xylazine	Bayer	N/A
tiletamine plus zolazepam	Virbac	N/A	veterinary drug
proparacaine hydrochloride ophthalmic solution	Alcon	N/A	veterinary drug
0.1% atropine	Wu-Fu Laboratories Co., Ltd	N/A	clinical drug
0.3% gentamicin sulfate	Sinphar Group	N/A	clinical drug
basic fibroblast growth factor	ThermoFisher Scientific	PHG0024	clinical drug

Referanslar

Maurice, D. M. The location of the fluid pump in the cornea. J Physiol. 221 (1), 43-54 (1972).
Joyce, N. Proliferative capacity of the corneal endothelium. Progress in Retinal and Eye Research. 22 (3), 359-389 (2003).
Morishige, N., Sonoda, K. H. Bullous keratopathy as a progressive disease: evidence from clinical and laboratory imaging studies. Cornea. 32, 77-83 (2013).
Bates, A. K., Cheng, H., Hiorns, R. W. Pseudophakic bullous keratopathy: relationship with endothelial cell density and use of a predictive cell loss model. A preliminary report. Curr Eye Res. 5 (5), 363-366 (1986).
Wilson, S. E., Lloyd, S. A. Epidermal growth factor and its receptor, basic fibroblast growth factor, transforming growth factor beta-1, and interleukin-1 alpha messenger RNA production in human corneal endothelial cells. Invest Ophthalmol Vis Sci. 32 (10), 2747-2756 (1991).
Chen, K. H., Harris, D. L., Joyce, N. C. TGF-beta2 in aqueous humor suppresses S-phase entry in cultured corneal endothelial cells. Invest Ophthalmol Vis Sci. 40 (11), 2513-2519 (1999).
Senoo, T., Obara, Y., Joyce, N. C. EDTA: a promoter of proliferation in human corneal endothelium. Invest Ophthalmol Vis Sci. 41 (10), 2930-2935 (2000).
Yue, B. Y., Sugar, J., Gilboy, J. E., Elvart, J. L. Growth of human corneal endothelial cells in culture. Invest Ophthalmol Vis Sci. 30 (2), 248-253 (1989).
Peh, G. S., Beuerman, R. W., Colman, A., Tan, D. T., Mehta, J. S. Human corneal endothelial cell expansion for corneal endothelium transplantation: an overview. Transplantation. 91 (8), 811-819 (2011).
Zhu, C., Rawe, I., Joyce, N. C. Differential protein expression in human corneal endothelial cells cultured from young and older donors. Mol Vis. 14, 1805-1814 (2008).
Ko, M. K., Kay, E. P. Regulatory role of FGF-2 on type I collagen expression during endothelial mesenchymal transformation. Invest Ophthalmol Vis Sci. 46 (12), 4495-4503 (2005).
Lee, H. T., Kay, E. P. FGF-2 induced reorganization and disruption of actin cytoskeleton through PI 3-kinase, Rho, and Cdc42 in corneal endothelial cells. Mol Vis. 9, 624-634 (2003).
Pipparelli, A., et al. ROCK Inhibitor Enhances Adhesion and Wound Healing of Human Corneal Endothelial Cells. PloS one. 8 (4), e62095 (2013).
Roy, O., Leclerc, V. B., Bourget, J. M., Theriault, M., Proulx, S. Understanding the process of corneal endothelial morphological change in vitro. Invest Ophthalmol Vis Sci. 56 (2), 1228-1237 (2015).
Jakobiec, F. A., Bhat, P. Retrocorneal membranes: a comparative immunohistochemical analysis of keratocytic, endothelial, and epithelial origins. Am J Ophthalmol. 150 (2), 230-242 (2010).
Okumura, N., et al. Involvement of ZEB1 and Snail1 in excessive production of extracellular matrix in Fuchs endothelial corneal dystrophy. Lab Invest. 95 (11), 1291-1304 (2015).
Okumura, N., et al. Enhancement on primate corneal endothelial cell survival in vitro by a ROCK inhibitor. Invest Ophthalmol Vis Sci. 50 (8), 3680-3687 (2009).
Zhu, Y. T., Chen, H. C., Chen, S. Y., Tseng, S. C. G. Nuclear p120 catenin unlocks mitotic block of contact-inhibited human corneal endothelial monolayers without disrupting adherent junctions. J Cell Sci. 125 (15), 3636-3648 (2012).
Ho, W. T., et al. Inhibition of Matrix Metalloproteinase Activity Reverses Corneal Endothelial-Mesenchymal Transition. Am J Pathol. 185 (8), 2158-2167 (2015).
Kay, E. D., Cheung, C. C., Jester, J. V., Nimni, M. E., Smith, R. E. Type I collagen and fibronectin synthesis by retrocorneal fibrous membrane. Invest Ophthalmol Vis Sci. 22 (2), 200-212 (1982).
Li, C., et al. Notch Signal Regulates Corneal Endothelial-to-Mesenchymal Transition. Am J Pathol. 183 (3), 786-795 (2013).
Okumura, N., et al. The ROCK Inhibitor Eye Drop Accelerates Corneal Endothelium Wound Healing. Invest Ophthalmol Vis Sci. 54 (4), 2493-2502 (2013).
Mannermaa, E., Vellonen, K. S., Urtti, A. Drug transport in corneal epithelium and blood-retina barrier: emerging role of transporters in ocular pharmacokinetics. Adv Drug Deliv Rev. 58 (11), 1136-1163 (2006).

Etiketler

Corneal Endothelial-mesenchymal Transition In Vitro In Vivo Corneal Endothelium Regeneration Bovine Eyes Descemet’s Membrane Corneal Endothelial Cells SHEM Trypsin Hemacytometer Maramastat Paraformaldehyde Triton X-100 BSA ABC Snail Slug

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Ho, W., Su, C., Chang, J., Chang, S., Hu, F., Jou, T., Wang, I. In Vitro and In Vivo Models to Study Corneal Endothelial-mesenchymal Transition. J. Vis. Exp. (114), e54329, doi:10.3791/54329 (2016).