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The influence of microtubule integrity on plasma membrane fluidity in L929 cells
Authors:Arlette Rémy-Kristensen  Guy Duportail  Gilliane Coupin  Jean-Georges Kuhry
Institution:1. Laboratoire de Pharmacologie et Physico-chimie, UMR CNRS 7034, France;2. Laboratoire d'Immunopharmacologie, Faculté de Pharmacie de Strasbourg, B.P. 24, 67401 Illkirch Cedex, France
Abstract:The aim of this work was to examine the possible influence of the integrity of the microtubule network on the plasma membrane fluidity of L929 mouse fibroblasts. The L929 cell line was selected for the ease of culture and the stability of its characteristics. The cells were treated with colchicine, nocodazole and vinblastine, three microtubule-depolymerizing drugs, at various concentrations and for various times. Membrane fluidity was assessed from fluorescence depolarization measurements with the plasma membrane probe TMA-DPH. Each of the drugs induced a significant, dose-dependent decrease in fluorescence anisotropy. The effect levelled off (5-7% decrease) after ~ 90 min of treatment, and could be unambiguously interpreted as resulting from an increase in membrane fluidity. The cumulative action of the drugs did not significantly increase the effect. The effects of colchicine and nocodazole could be reversed by incubation in drug-free medium, but not that of vinblastine. The results are discussed in correlation with the kinetics of the three drugs interaction with tubulin or microtubules. It is concluded that the microtubule integrity contributed to the high plasma membrane lipidic order, but less than other factors, like the lipid composition and the cholesterol content.
Keywords:Microtubules Cytoskeleton Membrane Fluidity Tma-DPH
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