Characterization of Growth and Differentiation in a Telomerase-Immortalized Human Corneal Epithelial Cell Line

doi:10.1167/iovs.04-0528

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(Investigative Ophthalmology and Visual Science. 2005;46:470-478.)
© 2005 by The Association for Research in Vision and Ophthalmology, Inc.
DOI: 10.1167/iovs.04-0528

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Characterization of Growth and Differentiation in a Telomerase-Immortalized Human Corneal Epithelial Cell Line

Danielle M. Robertson,¹ Li Li,¹ Stephen Fisher,¹ Virginia P. Pearce,² Jerry W. Shay,² Woodring E. Wright,² H. Dwight Cavanagh,¹ and James V. Jester¹

^¹From the Departments of Ophthalmology, and ^²Cell Biology, The University of Texas Southwestern Medical Center, Dallas, Texas.

PURPOSE. To develop and characterize a telomerase-immortalizedhuman corneal epithelial cell line (hTCEpi) to serve as an invitro model for studying the molecular mechanisms involved inregulating human corneal epithelial cell differentiation.

METHODS. Primary cultures of human corneal epithelial cellswere infected with a retroviral vector encoding human telomerasereverse transcriptase (hTERT). Infected hTCEpi cells were selected,cloned, and characterized to identify telomerase activity, proliferativecapacity, karyotype, and differentiative potential in routineculture and under consecutive submerged and air-lifted conditions.Cells were evaluated to measure cell cycle kinetics (anti-Ki-67,anti-p16), stratification (phalloidin and anti-ZO-1), and differentiation(anti-K3, anti-BCL-2 and TUNEL labeling).

RESULTS. hTCEpi cells exhibited telomerase activity, a normalkaryotype and cell cycle kinetics at greater than 240 populationdoublings, and loss of p16 after passage 10. Air-lifting produceda well stratified epithelium (five to seven cell layers) withapical ZO-1-stained tight junctions. Submersed culture demonstratedincreasing expression of stratification markers (K5/K14) withK3-corneal keratin marker expression in long-term, air-liftedculture. Anti-BCL-2 staining showed both nuclear and cytoplasmiclocalization with loss of nuclear BCL-2 expression in TUNEL-labeledsurface epithelial cells.

CONCLUSIONS. hTCEpi cells stratify, differentiate, and desquamatesimilar to normal human corneal epithelium. Further study ofthe hTCEpi cell line may be valuable in studying the molecularmechanisms regulating corneal epithelial cell differentiationand desquamation.

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