We studied responses of endothelial and epithelial cells in the thin portion of the air-blood barrier to a rise in interstitial pressure caused by an increase in extravascular water (interstitial edema) obtained in anesthetized rabbits receiving saline infusion (0.5 ml . kg(-1) . min(-1) for 3 h). We obtained morphometric analyses of the cells and of their microenvironment (electron microscopy); furthermore, we also studied in lung tissue extracts the biochemical alterations of proteins responsible for signal transduction (PKC, caveolin-1) and cell-cell adhesion (CD31) and of proteins involved in membrane-to-cytoskeleton linkage (alpha-tubulin and beta-tubulin). In endothelial cells, we observed a folding of the plasma membrane with an increase in cell surface area, a doubling of plasmalemma vesicular density, and an increase in cell volume. Minor morphological changes were observed in epithelial cells. Edema did not affect the total plasmalemma amount of PKC, beta-tubulin, and caveolin-1 but alpha-tubulin and CD-31 increased. In edema, the distribution of these proteins changed between the detergent-resistant fraction of the plasma membrane (DRF, lipid microdomains) and the rest of the plasma membrane [high-density fractions (HDFs)]. PKC and tubulin isoforms shifted from the DRF to HDFs in edema, whereas caveolin-1 increased in DRF at the expense of a decrease in phosphorylated caveolin-1. The changes in cellular morphology and in plasma membrane composition suggest an early endothelial response to mechanical stimuli arising at the interstitial level subsequently to a modest (similar to5%) increase in extravascular water.

Daffara, R., Botto, L., Beretta, E., Conforti, E., Faini, A., Palestini, P., et al. (2004). Endothelial cells as early sensors of pulmonary interstitial edema. JOURNAL OF APPLIED PHYSIOLOGY, 97(4), 1575-1583 [10.1152/japplphysiol.00236.2004].

Endothelial cells as early sensors of pulmonary interstitial edema

BOTTO, LAURA MARIA;Beretta, E;FAINI, ANDREA;PALESTINI, PAOLA NOVERINA ADA;MISEROCCHI, GIUSEPPE ANDREA
2004

Abstract

We studied responses of endothelial and epithelial cells in the thin portion of the air-blood barrier to a rise in interstitial pressure caused by an increase in extravascular water (interstitial edema) obtained in anesthetized rabbits receiving saline infusion (0.5 ml . kg(-1) . min(-1) for 3 h). We obtained morphometric analyses of the cells and of their microenvironment (electron microscopy); furthermore, we also studied in lung tissue extracts the biochemical alterations of proteins responsible for signal transduction (PKC, caveolin-1) and cell-cell adhesion (CD31) and of proteins involved in membrane-to-cytoskeleton linkage (alpha-tubulin and beta-tubulin). In endothelial cells, we observed a folding of the plasma membrane with an increase in cell surface area, a doubling of plasmalemma vesicular density, and an increase in cell volume. Minor morphological changes were observed in epithelial cells. Edema did not affect the total plasmalemma amount of PKC, beta-tubulin, and caveolin-1 but alpha-tubulin and CD-31 increased. In edema, the distribution of these proteins changed between the detergent-resistant fraction of the plasma membrane (DRF, lipid microdomains) and the rest of the plasma membrane [high-density fractions (HDFs)]. PKC and tubulin isoforms shifted from the DRF to HDFs in edema, whereas caveolin-1 increased in DRF at the expense of a decrease in phosphorylated caveolin-1. The changes in cellular morphology and in plasma membrane composition suggest an early endothelial response to mechanical stimuli arising at the interstitial level subsequently to a modest (similar to5%) increase in extravascular water.
Articolo in rivista - Articolo scientifico
Air-blood barrier; Mechanotransduction; Morphometry; Plasma membrane proteins; Pulmonary interstitial pressure;
English
2004
97
4
1575
1583
none
Daffara, R., Botto, L., Beretta, E., Conforti, E., Faini, A., Palestini, P., et al. (2004). Endothelial cells as early sensors of pulmonary interstitial edema. JOURNAL OF APPLIED PHYSIOLOGY, 97(4), 1575-1583 [10.1152/japplphysiol.00236.2004].
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/10281/1022
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