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Erythroid properties of K562 cells : Effect of hemin, butyrate and TPA induction
Authors:J L Villeval  P G Pelicci  A Tabilio  M Titeux  A Henri  F Houesche  P Thomopoulos  W Vainchenker  M Garbaz  H Rochant  J Breton-Gorius  P A W Edwards  U Testa
Institution:1. Unité INSERM U91, Hôpital Henri Mondor, 94010 Creteil, France;2. Unité INSERM U35, Hôpital Henri Mondor, 94010 Creteil, France;3. Ludwig Institute for Cancer Research (London Branch), The Haddow Laboratories, Royal Marsden Hospital, Sutton, Surrey, UK;4. Unité INSERM U160, Hôpital Beaujon, 92110 Clichy, France
Abstract:Two sublines of the human leukemia cell line K562 including the original cell line and three clones have been investigated for their erythroid features. All of them produce embryonic and fetal hemoglobins, glycophorin A, spectrin and true acetylcholinesterase, but to a varying extent among the cell lines. The Hb and glycophorin contents were correlated in the different K562 cell lines, whereas acetylcholinesterase was independently expressed from these two other erythroid markers. Hb accumulation is enhanced by exposure of the cells to 100 microM hemin without a significant modification of the expression of the other erythroid markers. Butyrate greatly increased the activity of acetylcholinesterase, slightly enhanced the production of hemoglobin, but did not modify the expression of glycophorin and spectrin. 12-O-tetradecanoyl-phorbol-13-acetate (TPA) induced an almost complete disappearance of glycophorin, reduced the synthesis of Hb by K562 cells and also abolished the action of hemin on Hb accumulation. Therefore, all the different K562 cell lines exhibit clear erythroid features including acetylcholinesterase. Butyrate or hemin did not induce terminal differentiation of K562 cells, whereas TPA significantly diminished the erythroid phenotype.
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