Characterisation of Lectin Binding Patterns of Mouse Bronchiolar and Rat Alveolar Epithelial Cells in Culture

被引:0
|
作者
Shirley McBride
Erzsebet Tatrai
Renald Blundell
Zuzana Kovacikova
Lorraine Cardozo
Zoltan Adamis
Tim Smith
David Harrison
机构
[1] University of Edinburgh Medical School,Department of Pathology
[2] National Institute of Occupational Health,MRC Toxicological Unit
[3] Institute of Preventive and Clinical Medicine,undefined
[4] National Institute of Chemical Safety,undefined
[5] University of Leicester,undefined
来源
The Histochemical Journal | 2000年 / 32卷
关键词
Alkaline Phosphatase Activity; Concanavalin; Wheat Germ; Alveolar Epithelial Cell; Mouse Lung;
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学科分类号
摘要
Lung epithelial cell differentiation pathways remain unclear. This is due in part to the plasticity of these cells and the lack of markers which accurately reflect their differentiation status. The aim of this study was to determine if lectin binding properties are useful determinants of functional differentiation status in vitro. Mouse Clara cells were cultured for 5 days. During this time, no alteration in differentiation was evident by electron microscopy. No significant alteration in binding reactivity of Bauhinia purpurea (BPA), Maclura pomifera (MPA), Concanavalin A, Wheat germ or Helix pomatia lectins occurred in cultures compared with Clara cells in mouse lung tissue. In contrast, nitrotetrazolium blue reductase activity and CC10 expression declined in culture. Rat type II cells were cultured for 8 days. Between days 0 and 4, the number of type II cells identified by electron microscopy was constant at 70–80%, decreasing to 8% by day 6. In contrast, by day 4, only 42% cells retained alkaline phosphatase activity. BPA and MPA reactivity was altered at day 0 and day 4 respectively, compared with cells in situ. Therefore, the reactivity of lectins analysed here does not reflect functional differentiation status of cultured mouse Clara cells. However, BPA and MPA reactivity may be a sensitive indicator of alterations in rat type II cell differentiation in vitro.
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页码:33 / 40
页数:7
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