• 主题
高级搜索  >
历史搜索 清空历史
首页> 美国卫生研究院文献>Journal of Hematology Oncology >Proliferation inhibition and apoptosis induction of imatinib-resistant chronic myeloid leukemia cells via PPP2R5C down-regulation
【2h】

Proliferation inhibition and apoptosis induction of imatinib-resistant chronic myeloid leukemia cells via PPP2R5C down-regulation

机译:PPP2R5C下调对伊马替尼耐药的慢性粒细胞白血病细胞的增殖抑制和凋亡诱导作用

代理获取
本网站仅为用户提供外文OA文献查询和代理获取服务,本网站没有原文。下单后我们将采用程序或人工为您竭诚获取高质量的原文,但由于OA文献来源多样且变更频繁,仍可能出现获取不到、文献不完整或与标题不符等情况,如果获取不到我们将提供退款服务。请知悉。
页面导航
  • 摘要
  • 著录项
  • 相似文献
  • 相关主题

摘要

Despite the success of imatinib and other tyrosine kinase inhibitors (TKIs), chronic myeloid leukemia (CML) remains largely incurable, and a number of CML patients die due to Abl mutation-related drug resistance and blast crisis. The aim of this study was to evaluate proliferation inhibition and apoptosis induction by down-regulating PPP2R5C gene expression in the imatinib-sensitive and imatinib-resistant CML cell lines K562, K562R (imatinib resistant without an Abl gene mutation), 32D-Bcr-Abl WT (imatinib-sensitive murine CML cell line with a wild type Abl gene) and 32D-Bcr-Abl T315I (imatinib resistant with a T315I Abl gene mutation) and primary cells from CML patients by RNA interference. PPP2R5C siRNAs numbered 799 and 991 were obtained by chemosynthesis. Non-silencing siRNA scrambled control (SC)-treated, mock-transfected, and untreated cells were used as controls. The PPP2R5C mRNA and protein expression levels in treated CML cells were analyzed by quantitative real-time PCR and Western blotting, and in vitro cell proliferation was assayed with the cell counting kit-8 method. The morphology and percentage of apoptosis were revealed by Hoechst 33258 staining and flow cytometry (FCM). The results demonstrated that both siRNAs had the best silencing results after nucleofection in all four cell lines and primary cells. A reduction in PPP2R5C mRNA and protein levels was observed in the treated cells. The proliferation rate of the PPP2R5C-siRNA-treated CML cell lines was significantly decreased at 72 h, and apoptosis was significantly increased. Significantly higher proliferation inhibition and apoptosis induction were found in K562R cells treated with PPP2R5C-siRNA799 than K562 cells. In conclusion, the suppression of PPP2R5C by RNA interference could inhibit proliferation and effectively induce apoptosis in CML cells that were either imatinib sensitive or resistant. Down-regulating PPP2R5C gene expression might be considered as a new therapeutic target strategy for CML, particularly for imatinib-resistant CML.
机译:尽管伊马替尼和其他酪氨酸激酶抑制剂(TKIs)取得了成功,但慢性髓细胞性白血病(CML)仍基本无法治愈,许多CML患者由于与Abl突变相关的耐药性和瘟疫危机而死亡。这项研究的目的是通过下调PPP2R5C基因在伊马替尼敏感和伊马替尼耐药的CML细胞系K562,K562R(无Abl基因突变的伊马替尼耐药),32D-Bcr-Abl中评估增殖抑制和凋亡诱导WT(具有野生型Abl基因的伊马替尼敏感性鼠CML细胞系)和32D-Bcr-Abl T315I(具有T315I Abl基因突变的伊马替尼耐药)和来自CML患者的原代细胞,通过RNA干扰。通过化学合成获得了编号为799和991的PPP2R5C siRNA。使用非沉默siRNA加扰对照(SC)处理,模拟转染和未处理的细胞作为对照。通过定量实时PCR和Western印迹分析处理过的CML细胞中的PPP2R5C mRNA和蛋白表达水平,并用细胞计数试剂盒8法测定体外细胞增殖。 Hoechst 33258染色和流式细胞仪(FCM)揭示了细胞凋亡的形态学和百分比。结果表明,在所有四个细胞系和原代细胞中,两种siRNA在核转染后均具有最佳的沉默效果。在处理的细胞中观察到PPP2R5C mRNA和蛋白质水平的降低。 PPP2R5C-siRNA处理的CML细胞系在72小时的增殖速率显着降低,并且凋亡显着增加。在用PPP2R5C-siRNA799处理的K562R细胞中,发现其增殖抑制和凋亡诱导作用明显高于K562细胞。总之,RNA干扰抑制PPP2R5C可以抑制增殖,并有效诱导对伊马替尼敏感或耐药的CML细胞凋亡。下调PPP2R5C基因表达可能被认为是CML的新治疗靶标策略,尤其是对伊马替尼耐药的CML。

著录项

相似文献

  • 外文文献
  • 中文文献
  • 专利
代理获取

客服邮箱:kefu@zhangqiaokeyan.com

京公网安备:11010802029741号 ICP备案号:京ICP备15016152号-6 六维联合信息科技 (北京) 有限公司©版权所有

  • 客服微信

  • 服务号