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Suppression of bcr‐abl synthesis by siRNAs or tyrosine kinase activity by Glivec alters different oncogenes, apoptotic/antiapoptotic genes and cell proliferation factors (microarray study)
Author(s) -
Zhelev Zhivko,
Bakalova Rumiana,
Ohba Hideki,
Ewis Ashraf,
Ishikawa Mitsuru,
Shinohara Yasuo,
Baba Yoshinobu
Publication year - 2004
Publication title -
febs letters
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.593
H-Index - 257
eISSN - 1873-3468
pISSN - 0014-5793
DOI - 10.1016/j.febslet.2004.06.048
Subject(s) - small interfering rna , microbiology and biotechnology , tyrosine kinase , biology , chronic myelogenous leukemia , oncogene , cancer research , breakpoint cluster region , k562 cells , transfection , abl , chemistry , cell , cell cycle , signal transduction , leukemia , gene , immunology , biochemistry
Short 21‐mer double‐stranded/small‐interfering RNAs (ds/siRNAs) were designed to target bcr‐abl mRNA in chronic myelogenous leukemia. The ds/siRNAs were transfected into bcr‐abl‐positive K‐562 (derived from blast crisis chronic myelogenous leukemia), using lipofectamine. Penetrating of ds/siRNAs into the cells was detected by fluorescent confocal microscopy, using fluorescein‐labeled ds/siRNAs. The cells were treated with mix of three siRNA sequences (3 × 60 nM) during 6 days with three repetitive transfections. The siRNA‐treatment was accompanied with significant reduction of bcr‐abl mRNA, p210, protein tyrosine kinase activity and cell proliferation index. Treatment of cells with Glivec (during 8 days with four repetitive doses, 180 nM single dose) resulted in analogous reduction of cell proliferation activity, stronger suppression of protein tyrosine kinase activity, and very low reduction of p210. siRNA‐mix and Glivec did not affect significantly the viability of normal lymphocytes. Microarray analysis of siRNA‐ and Glivec‐treated K‐562 cells demonstrated that both pathways of bcr‐abl suppression were accompanied with overexpression and suppression of many different oncogenes, apoptotic/antiapoptotic and cell proliferation factors. The following genes of interest were found to decrease in relatively equal degree in both siRNA‐ and Glivec‐treated cells: Bcd orf1 and orf2 proto‐oncogene, chromatin‐specific transcription elongation factor FACT 140‐kDa subunit mRNA, gene encoding splicing factor SF1, and mRNA for Tec protein tyrosine kinase. siRNA‐mix and Glivec provoked overexpression of the following common genes: c‐jun proto‐oncogene, protein kinase C‐α, pvt‐1 oncogene homologue (myc activator), interleukin‐6, 1‐8D gene from interferon‐inducible gene family, tumor necrosis factor receptor superfamily (10b), and STAT‐induced STAT inhibitor.

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