Ann Tisdale scite author profile

Antisera that recognize the a6 and (34 subunits of integrins were found by immunoelectron microscopy to localize to hemidesmosomes in the basal cells of mouse corneal epithelium. Immunoprecipitation experiments using extracts of metabolically labeled corneal epithelial cells indicate that the primary a6-subunit-containing integrin heterodimer present is a434 and not a6431. Here we extend previous studies to report that by immunofluorescence microscopy the a6 integrin subunit colocalizes with bullous pemphigoid antigen and type V1I collagen in newly forming hemidesmosomes in the developing 17-day fetal rabbit eye. Neither the composition of the anchoring filaments, which span the region between the hemidesmosomal plaque and the lamina densa of basement membrane where the globular domain of type VII collagen is located, nor the extracellular ligand of a6.84 is known. Once anchoring filament proteins are identified, it will be of interest to determine whether any bind to a484.Hemidesmosomes are cell-substrate adhesionjunctions present along the basal cell-basement membrane junction of stratified squamous epithelia (1,2). By comparison to desmosomes, biochemical characterization of the basic components of the hemidesmosome has been slow, due in part to difficulty in obtaining hemidesmosome-enriched cellular fractions. The only characterized component of the hemidesmosome is the bullous pemphigoid antigen (BPA), a 230-kDa protein present in the cytoplasmic plaque of the hemidesmosome (3-5). BPA is found within the electron-dense cytoplasmic plaque region of the hemidesmosome. The sequence of cDNA clones encoding the BPA molecule, although not entirely complete, shows no integral membrane segment (J. Stanley, personal communication). Several other monoclonal antibodies specific to hemidesmosomes have been reported, and their antigens await characterization (6, 7). Clearly, other molecules are present in both the cytoplasmic and the extracellular aspect of the hemidesmosome.The molecule(s) that traverses the cell membrane in hemidesmosomes has yet to be identified; candidates include members of the integrin superfamily of extracellular matrix receptors (8-12). The integrins are integral membrane glycoproteins that function as cell-cell and cell-substrate adhesion molecules. As a result of our studies to localize and characterize integrin subunits present in corneal epithelium, we noted that antibodies to both the a6 and (4 integrin subunits bound to the basal cell-basement membrane zone in stationary epithelia. This prompted us to determine whether the heterodimer is associated with hemidesmosomes. The present study reports that a6 and P4 integrins colocalize with BPA and type VII collagen in hemidesmosomes of developing epithelia, that both a6 and (3 antibodies bind to hemidesmosomes as shown by immunoelectron microscopy, and that both a434 and a43l heterodimers can be identified in epithelia by immunoprecipitation. MATERIALS AND METHODSTissue Preparation. For adult corneal epithelium, New Zealand White (NZW) ...

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Goblet Cell Numbers and Epithelial Proliferation in the Conjunctiva of Patients With Dry Eye Syndrome Treated With Cyclosporine

Kunert

Tisdale²,

Gipson³

2002

Arch Ophthalmol

318

201

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To compare conjunctival goblet cell numbers as well as epithelial turnover in patients with non-Sjö gren syndrome-associated keratoconjunctivitis sicca (NSS-KCS) and those with SS-KCS before and after 6 months of treatment with topical cyclosporine A (CsA) ophthalmic emulsion.Methods: Conjunctival biopsy specimens from 16 patients with NSS-KCS and 12 with SS-KCS were obtained at baseline and after 6 months' therapy with CsA or vehicle alone. Conjunctival biopsy specimens were also obtained from 11 normal subjects. Periodic acid-Schiff staining determined the number of goblet cells present. Immunofluorescence microscopy for Ki-67 localization was used to evaluate the number of actively cycling cells.Results: Periodic acid-Schiff staining showed fewer goblet cells at baseline in both dry eye populations when compared with normal subjects (PϽ.001). After 6 months of CsA treatment, conjunctival biopsy specimens of both NSS-KCS and SS-KCS groups revealed an increase in goblet cells compared with baseline (PϽ.05). More Ki-67positive cells were observed in NSS-KCS conjunctiva at baseline than in normal conjunctiva (PϽ.05) whereas numbers of these cells in SS-KCS conjunctiva were similar to normal at baseline. After 6 months of CsA treatment, conjunctival biopsy specimens of NSS-KCS revealed a decrease in Ki-67-labeled cells compared with baseline (PϽ.001). In contrast, no substantial change was observed for CsA treatment in patients with SS-KCS.Conclusions: Treatment of dry eye syndrome for 6 months with topical CsA resulted in an increase in goblet cell numbers in patients with NSS-KCS and SS-KCS and a decrease in epithelial turnover in those with NSS-KCS. Reducing ocular surface inflammation might have an effect on the proliferative activity of the epithelium.

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Ann Tisdale

Mucin Gene Expression in Immortalized Human Corneal–Limbal and Conjunctival Epithelial Cell Lines

Alpha 6 beta 4 integrin heterodimer is a component of hemidesmosomes.

Goblet Cell Numbers and Epithelial Proliferation in the Conjunctiva of Patients With Dry Eye Syndrome Treated With Cyclosporine

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