Literature DB >> 1572908

Proliferative and differentiative response of corneal and limbal epithelium to extracellular calcium in serum-free clonal cultures.

F E Kruse1, S C Tseng.   

Abstract

An increasing concentration of extracellular Ca2+ ([Ca2+]e) consistently induces epithelial differentiation, but its effect on proliferation remains variable. We investigated the effect of [Ca2+]e on two different cell populations: the peripheral corneal (PC) and limbal (L) epithelia, the latter containing corneal stem cells. Primary clonal (18 cells/cm2) cultures from rabbit limbal and peripheral corneal epithelia were established in serum-free MCDB 151 medium containing growth-promoting agents and 0.03, 0.3, or 1.8 mM Ca2+. During early culture life, colony size and the BrdU labelling-index of L and PC, assayed on day 6, increased in response to increasing [Ca2+]e; cell attachment and colony-forming efficiency remained unchanged for both L and PC epithelia. These results indicate that increasing [Ca2+]e, under these defined conditions, stimulates the proliferation of transient amplifying cells, but does not stimulate the differentiation of stem cells into clonal proliferation. A 10-fold increase of the seeding density or prolongation of the culture up to day 14 or 21 changed the response to [Ca2+]e allowing better proliferation in lower [Ca2+]e. Only cells grown as a monolayer in 0.03 mM Ca2+ could still be passaged on day 14, whereas cells in higher [Ca2+]e showed increasing stratification and cell detachment and could not be passaged. Normal cellular differentiation accessed by the expression of a cornea-type K3 keratin, recognized by the monoclonal antibody AE-5, was enhanced by increasing [Ca2+]e. Abnormal differentiation featured by the formation of cornified envelopes was only observed in higher [Ca2+]e. These results indicate that [Ca2+]e promotes the proliferation of relatively undifferentiated transient amplifying cells under clonal, serum-free culture conditions. Factors that enhance differentiation, such as seeding density or prolonged culture life, can modify this response and allow better proliferation in low [Ca2+]e.

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Year:  1992        PMID: 1572908     DOI: 10.1002/jcp.1041510216

Source DB:  PubMed          Journal:  J Cell Physiol        ISSN: 0021-9541            Impact factor:   6.384


  6 in total

1.  The effect of hydrocortisone and thyroxine on development of calcium homeostasis in embryonic intestinal epithelium.

Authors:  J O Rogers; B L Black
Journal:  Experientia       Date:  1996-06-15

2.  Comparison of culture media indicates a role for autologous serum in enhancing phenotypic preservation of rabbit limbal stem cells in explant culture.

Authors:  Mehmet Gürdal; Özlem Barut Selver; Kemal Baysal; İsmet Durak
Journal:  Cytotechnology       Date:  2017-12-04       Impact factor: 2.058

3.  Activation of Smad-mediated TGF-β signaling triggers epithelial-mesenchymal transitions in murine cloned corneal progenitor cells.

Authors:  Tetsuya Kawakita; Edgar M Espana; Kazunari Higa; Naoko Kato; Wei Li; Scheffer C G Tseng
Journal:  J Cell Physiol       Date:  2013-01       Impact factor: 6.384

Review 4.  Stem cells treatment in the ocular surface regeneration.

Authors:  Cristina Nicula; Izabela Szabo; Ozana Ivan
Journal:  Rom J Ophthalmol       Date:  2017 Oct-Dec

5.  The Effect of Calcium and Glucose Concentration on Corneal Epithelial Cell Lines Differentiation, Proliferation, and Focal Adhesion Expression.

Authors:  Sophia Masterton; Mark Ahearne
Journal:  Biores Open Access       Date:  2019-06-05

6.  Comparison of culture media for ex vivo cultivation of limbal epithelial progenitor cells.

Authors:  Renata Ruoco Loureiro; Priscila Cardoso Cristovam; Caio Marques Martins; Joyce Luciana Covre; Juliana Aparecida Sobrinho; José Reinaldo da Silva Ricardo; Rossen Myhailov Hazarbassanov; Ana Luisa Höfling-Lima; Rubens Belfort; Mauro Nishi; José Álvaro Pereira Gomes
Journal:  Mol Vis       Date:  2013-01-17       Impact factor: 2.367

  6 in total

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