September 1998
Volume 39, Issue 10
Free
Articles  |   September 1998
Isolation, culture, and characterization of endothelial cells from Schlemm's canal.
Author Affiliations
  • W D Stamer
    Department of Ophthalmology, Duke University Medical Center and Veterans Affairs Medical Center, Durham, North Carolina 27710-3802, USA.
  • B C Roberts
    Department of Ophthalmology, Duke University Medical Center and Veterans Affairs Medical Center, Durham, North Carolina 27710-3802, USA.
  • D N Howell
    Department of Ophthalmology, Duke University Medical Center and Veterans Affairs Medical Center, Durham, North Carolina 27710-3802, USA.
  • D L Epstein
    Department of Ophthalmology, Duke University Medical Center and Veterans Affairs Medical Center, Durham, North Carolina 27710-3802, USA.
Investigative Ophthalmology & Visual Science September 1998, Vol.39, 1804-1812. doi:
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      W D Stamer, B C Roberts, D N Howell, D L Epstein; Isolation, culture, and characterization of endothelial cells from Schlemm's canal.. Invest. Ophthalmol. Vis. Sci. 1998;39(10):1804-1812.

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Abstract

PURPOSE: An important goal in glaucoma research has been to understand the functional contribution of trabecular meshwork (TM) and Schlemm's canal (SC) endothelia to aqueous humor outflow resistance. To date, TM cells are routinely cultured and used as a model by several laboratories. However, there has been only limited success in isolating SC cells. The current objective was to develop a technique for selective isolation and culture of endothelial cells from human SC. METHODS: The anterior chamber of human cadaveric eyes was cut into eight equal and radially symmetric wedge-shaped pieces. Using a dissecting microscope, a gelatin-coated suture (6-0 sterile nylon monofilament) was gently inserted into the lumen of SC and advanced into the canal. The cannulated pieces of tissue were placed in culture medium and maintained for 3 weeks. Sutures were removed from SC and cells seeded onto 3-cm culture plates. Morphology, growth characteristics, and expression of endothelial surface antigens and other cellular markers were evaluated. RESULTS: Of the 20 pairs of eyes that were cannulated, primary cells were obtained from 13. All SC cell isolates had a fusiform morphology; formed nonoverlapping, linearly arranged monolayers; and were contact inhibited. Schlemm's canal cell isolates reacted with antibodies specific for CD44 (hyaluron receptor), CD54 (intercellular adhesion molecule-1, ICAM-1), tissue-type plasminogen activator, and TM-inducible glucocorticoid-responsive protein-myocilin (TIGR-MYOC). Unlike TM cells, however, TIGR-MYOC protein was not induced in SC cells after long-term dexamethasone treatment. Schlemm's canal cells endocytosed low-density lipoprotein and acetylated low-density lipoprotein, and in the presence of Matrigel organized into multicellular tubelike structures. CONCLUSIONS: Cannulation of SC with gelatin-coated suture material is an effective method for the isolation of human SC cells and provides a cellular model to study the potential role of SC cells in aqueous humor outflow function.

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