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Active cell membrane mechanisms involved in the exclusion of RH 123 allow distinction between normal and tumoral cells
Authors:G. Lizard  M. -C. Chignol  Y. Chardonnet  D. Schmitt
Affiliation:(1) Centre Commun de Cytométrie en Flux, INSERM U80, Hôpital E. Herriot, Pavillon P, 69437 Lyon Cédex 03, France;(2) INSERM U346, Affilliée CNRS, Hôpital E. Herriot, Pavillon R, 69437 Lyon Cédex 03, France;(3) CHRU du Bocage BP 1542, INSERM CJF 93-10, 21034 Dijon Cédex, France
Abstract:Human cell lines derived from three epithelial carcinomas (CaSki, HeLa, SiHa), one B lymphoma (BL60), one promyelocytic (HL60), one monocytic (U937) leukemia, one chronic myelogenous leukemia (sensitive K562S; multichemoresistant K562R) and normal human skin fibroblasts were compared for their capacity of staining with rhodamine 123 (Rh 123) and their kinetics of dye exclusion. Cells were exposed for 30 min to 10 mgrg/ml of Rh 123 in culture medium; fluorescence intensity was measured by flow cytometry immediately or 1, 2, 3 and 4 h after staining. The highest fluorescence intensity was observed in carcinoma cell lines; there was no incorporation in multichemoresistant K562R cells. Exclusion of Rh 123 was evaluated from 0 to 4 h, both by flow cytometry and by fluorimetry. Fluorescence intensity measured by flow cytometry decreased slightly in carcinoma and leukemia cells and rapidly in fibroblasts. In all cell lines Rh 123 exclusion was inhibited by 40 mgrmol/L verapamil and 5 mmol/L probenecid. Thus, incorporation and exclusion of Rh 123 allows distinction between normal and tumoral cells; moreover, inhibition of exclusion by verapamil and probenecid favors the involvement of active cell membrane mechanisms in the exclusion process.Abbreviations PBS phosphate-buffered saline - Rh 123 rhodamine 123
Keywords:cell membrane mechanisms  normal cells  probenecid  rhodamine 123  tumoral cells  verapamil
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