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阿糖胞苷耐药的急性髓系白血病细胞中脱氧胞苷激酶的表达缺陷

Defective expression of deoxycytidine kinase in cytarabine-resistant acute myeloid leukemia cells.

作者信息

Song Ju Han, Kim Seung Hyun, Kweon Sin Ho, Lee Tae Hyang, Kim Hee-Je, Kim Hyeoung-Joon, Kim Tae Sung

机构信息

Division of Life Sciences, School of Life Sciences and Biotechnology, Korea University, Seoul 136-701, Korea.

出版信息

Int J Oncol. 2009 Apr;34(4):1165-71. doi: 10.3892/ijo_00000245.

DOI:10.3892/ijo_00000245
PMID:19287976
Abstract

Resistance to cytarabine (Ara-C) incapacitates the therapeutic effort during the treatment of acute myeloid leukemia (AML). To elucidate mechanism responsible for the development of resistance to Ara-C, we established the Ara-C resistant AML-2/WT cell sublines, AML-2/IDAC and AML-2/ARC. We then conducted DNA microarray analysis to compare the AML-2/IDAC cells with parental AML-2/WT cells. The results of the microarray analysis revealed a severe defect in the expression of deoxycytidine kinase (dCK), which plays a key role in the transformation of Ara-C to the active form in AML-2/IDAC cells. A similar event was observed in AML-2/ARC cells, but not in Ara-C sensitive AML-2/IDA cells that were resistant to idarubicin. The decreased expression of dCK also resulted in lower activity in both Ara-C resistant variants. However, no significant difference in the intracellular concentration of Ara-C was observed among the cells tested, which indicates that the Ara-C resistant phenotype in our models occurred due to the lower expression and activity of dCK rather than a change in the ability to take up Ara-C. Additionally, in vitro assays using BM cells from AML patients revealed that the expression of dCK and the sensitivity to Ara-C were correlated. Taken together, these findings demonstrate that dCK can regulate the in vitro cellular response to Ara-C in AML cells.

摘要

对阿糖胞苷(Ara-C)的耐药性使急性髓系白血病(AML)治疗中的治疗效果大打折扣。为阐明对Ara-C产生耐药性的机制,我们建立了Ara-C耐药的AML-2/WT细胞亚系,即AML-2/IDAC和AML-2/ARC。然后我们进行了DNA微阵列分析,以比较AML-2/IDAC细胞与亲代AML-2/WT细胞。微阵列分析结果显示,脱氧胞苷激酶(dCK)的表达存在严重缺陷,dCK在AML-2/IDAC细胞中将Ara-C转化为活性形式的过程中起关键作用。在AML-2/ARC细胞中也观察到了类似情况,但在对伊达比星耐药的Ara-C敏感AML-2/IDA细胞中未观察到。dCK表达降低也导致两种Ara-C耐药变体的活性降低。然而,在所测试的细胞中未观察到Ara-C细胞内浓度的显著差异,这表明我们模型中的Ara-C耐药表型是由于dCK的低表达和活性,而非摄取Ara-C能力的改变所致。此外,使用AML患者骨髓细胞进行的体外试验表明,dCK的表达与对Ara-C的敏感性相关。综上所述,这些发现表明dCK可调节AML细胞对Ara-C的体外细胞反应。

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