Literature DB >> 19218612

Long-term culture and growth kinetics of murine corneal epithelial cells expanded from single corneas.

Xiaoli Ma1, Shigeto Shimmura, Hideyuki Miyashita, Satoru Yoshida, Miyuki Kubota, Tetsuya Kawakita, Kazuo Tsubota.   

Abstract

PURPOSE: To develop a reproducible procedure for the long-term culture of corneal epithelial cells from a single mouse cornea.
METHODS: Corneal limbal explants of C57BL6/J mice were cultured in serum-free, low-Ca(2+) medium supplemented with EGF and cholera toxin. Epithelial cells were subcultured at a 1:3 split until passage (P)4 and at lower densities after P4. Colony-forming efficiency, population-doubling times, and population doublings were determined. The expression of p63, keratin (K)19, K12, and involucrin was analyzed by RT-PCR, immunocytochemistry, and Western blotting. Differentiation potential was examined by switching the medium to serum or high Ca(2+)-containing medium. Stratification ability was analyzed by air-lift culture.
RESULTS: Thirty of 32 (93.8%) corneal explants were successfully subcultured to P1. Cultures without cholera toxin did not proliferate past P2 (n = 12), but 55% of cultures supplemented with cholera toxin achieved P4 (n = 20). After P4, cells were stably subcultured over 25 passages. Colony-forming efficiency increased from 9.7% +/- 2.6% at P5 to 29.0% +/- 3.3% at P20. The cells showed cobblestone appearance and expressed p63, K19, and involucrin but were negative for K12. Serum and high Ca(2+) induced differentiation, and cells cultured in DMEM/F12 with serum showed K12 mRNA expression. Stratified epithelium was formed by air-lifting.
CONCLUSIONS: With this procedure, corneal epithelial cells from a single cornea can be cultured long term and can retain the potential to differentiate and stratify. This procedure can be a powerful tool for studies that require comparison of corneal epithelial cells from normal and transgenic mice in vitro.

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Year:  2009        PMID: 19218612     DOI: 10.1167/iovs.08-2139

Source DB:  PubMed          Journal:  Invest Ophthalmol Vis Sci        ISSN: 0146-0404            Impact factor:   4.799


  16 in total

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4.  Behavioral heterogeneity of adult mouse lung epithelial progenitor cells.

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5.  Influence of Vitamin D on Corneal Epithelial Cell Desmosomes and Hemidesmosomes.

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Journal:  Invest Ophthalmol Vis Sci       Date:  2019-10-01       Impact factor: 4.799

6.  Effect of calcium on the proliferation and differentiation of murine corneal epithelial cells in vitro.

Authors:  Xiao-Li Ma; Han-Qiang Liu
Journal:  Int J Ophthalmol       Date:  2011-06-18       Impact factor: 1.779

7.  Effect of hypoxia on the proliferation of murine cornea limbal epithelial progenitor cells in vitro.

Authors:  Xiao-Li Ma; Han-Qiang Liu
Journal:  Int J Ophthalmol       Date:  2011-04-18       Impact factor: 1.779

8.  New technique for culturing corneal epithelial cells of normal mice.

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Journal:  Mol Vis       Date:  2009-08-14       Impact factor: 2.367

9.  Nucleostemin as a possible progenitor marker of corneal epithelial cells.

Authors:  Motoko Kawashima; Tetsuya Kawakita; Satoru Yoshida; Shigeto Shimmura; Kazuo Tsubota
Journal:  Mol Vis       Date:  2009-06-10       Impact factor: 2.367

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