Helena Sabanai scite author profile

Abstract. The integrity of the endothelial layer, which lines the entire cavity of the vascular system, depends on tight adhesion of the cells to the underlying basement membrane as well as to each other. It has been previously shown that such interactions occur via membrane receptors that determine the specificity, topology, and mechanical properties of the surface adhesion. Cell-cell junctions between endothelial cells, in culture and in situ, involve both Ca2+-dependent and -independent mechanisms that are mediated by distinct adhesion molecules. Ca2+-dependent cell-cell adhesion occurs mostly via members of the cadherin family, which locally anchor the microfilament system to the plasma membrane, in adherens junctions. Ca2+-independent adhesions were reported to mainly involve members of the Ig superfamily.In this study, we performed three-dimensional microscopic analysis of the relative subcellular distributions of these two endothelial intercellular adhesion systems. We show that cadherins are located at adjacent (usually more apical), yet clearly distinct domains of the lateral plasma membrane, compared to PECAM-1. Moreover, cadherins were first organized in adherens junctions within 2 h after seeding of endothelial cells, forming multiple lateral patches which developed into an extensive belt-like structure over a period of 24 h. PECAM-1 became associated with surface adhesions significantly later and became progressively associated with the cadherin-containing adhesions. Cadherins and PECAM-1 also differed in their detergent extractability, reflecting differences in their mode of association with the cytoskeleton. Moreover, the two adhesion systems could be differentially modulated since short treatment with the Ca 2+ chelator EGTA, disrupted the cadherin junctions leaving PECAM-1 apparently intact.These results confirm that endothelial cells possess distinct intercellular contact mechanisms that differ in their spatial and temporal organization as well as in their functional properties.

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Immuno-electron-microscopic localization of A-CAM in lens epithelial cells growing in low Ca2+ medium

Volk¹,

Sabanai²,

Geiger³

1988

Ultramicroscopy

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Helena Sabanai

Spatial and temporal relationships between cadherins and PECAM-1 in cell-cell junctions of human endothelial cells.

Immuno-electron-microscopic localization of A-CAM in lens epithelial cells growing in low Ca2+ medium

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