p27(Kip1) 在达沙替尼增强紫杉醇细胞毒性中的作用。
The role of p27(Kip1) in dasatinib-enhanced paclitaxel cytotoxicity in human ovarian cancer cells.
机构信息
Department of Experimental Therapeutics, the University of Texas M. D. Anderson Cancer Center, Unit 354, Rm Y6.5343, 1515 Holcombe Blvd, Houston, TX, USA.
出版信息
J Natl Cancer Inst. 2011 Sep 21;103(18):1403-22. doi: 10.1093/jnci/djr280. Epub 2011 Aug 2.
BACKGROUND
Less than 50% of ovarian cancers respond to paclitaxel. Effective strategies are needed to enhance paclitaxel sensitivity.
METHODS
A library of silencing RNAs (siRNAs) was used to identify kinases that regulate paclitaxel sensitivity in human ovarian cancer SKOv3 cells. The effect of dasatinib, an inhibitor of Src and Abl kinases, on paclitaxel sensitivity was measured in ovarian cancer cells and HEY xenografts. The roles of p27(Kip1), Bcl-2, and Cdk1 in apoptosis induced by dasatinib and paclitaxel were assessed using a terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL) assay, siRNA knockdown of gene expression, transfection with Bcl-2 and Cdk1 expression vectors, and flow cytometry. All statistical tests were two-sided.
RESULTS
Src family and Abl kinases were identified as modulators of paclitaxel sensitivity in SKOv3 cells. The siRNA knockdown of Src, Fyn, or Abl1 enhanced paclitaxel-mediated growth inhibition in ovarian cancer cells compared with a control siRNA. HEY cells treated with dasatinib plus paclitaxel formed fewer colonies than did cells treated with either agent alone. Treatment of HEY xenograft-bearing mice with dasatinib plus paclitaxel inhibited tumor growth more than treatment with either agent alone (average tumor volume per mouse, dasatinib + paclitaxel vs paclitaxel: 0.28 vs. 0.81 cm3, difference = 0.53 cm3, 95% confidence interval [CI] = 0.44 to 0.62 cm3, P = .014); dasatinib + paclitaxel vs. dasatinib: 0.28 vs. 0.55 cm3, difference = 0.27 cm3, 95% CI = 0.21 to 0.33 cm3, P = .035). Combined treatment induced more TUNEL-positive apoptotic cells than did either agent alone. The siRNA knockdown of p27(Kip1) decreased dasatinib- and paclitaxel-induced apoptosis compared with a negative control siRNA (sub-G1 fraction, control siRNA vs. p27(Kip1) siRNA: 42.5% vs. 20.1%, difference = 22.4%, 95% CI = 20.1% to 24.7%, P = .017). Studies with forced expression and siRNA knockdown of Bcl-2 and Cdk1 suggest that dasatinib-mediated induction of p27(Kip1) enhanced paclitaxel-induced apoptosis by negatively regulating Bcl-2 and Cdk1 expression.
CONCLUSION
Inhibition of Src family and Abl kinases with either siRNAs or dasatinib enhances paclitaxel sensitivity of ovarian cancer cells through p27(Kip1)-mediated suppression of Bcl-2 and Cdk1 expression.
背景
不到 50%的卵巢癌对紫杉醇有反应。需要有效的策略来增强紫杉醇的敏感性。
方法
使用沉默 RNA(siRNA)文库来鉴定调节人卵巢癌细胞 SKOv3 中紫杉醇敏感性的激酶。在卵巢癌细胞和 HEY 异种移植瘤中,测量Src 和 Abl 激酶抑制剂达沙替尼对紫杉醇敏感性的影响。使用末端脱氧核苷酸转移酶介导的 dUTP 缺口末端标记 (TUNEL) 测定、基因表达的 siRNA 敲低、Bcl-2 和 Cdk1 表达载体的转染以及流式细胞术评估达沙替尼和紫杉醇诱导的凋亡中 p27(Kip1)、Bcl-2 和 Cdk1 的作用。所有统计检验均为双侧检验。
结果
Src 家族和 Abl 激酶被鉴定为 SKOv3 细胞中紫杉醇敏感性的调节剂。与对照 siRNA 相比,Src、Fyn 或 Abl1 的 siRNA 敲低增强了卵巢癌细胞中紫杉醇介导的生长抑制。与单独使用任何一种药物相比,用达沙替尼加紫杉醇处理的 HEY 细胞形成的集落更少。与单独使用任何一种药物相比,用达沙替尼加紫杉醇治疗荷瘤 HEY 异种移植小鼠抑制肿瘤生长的效果更好(每只小鼠的平均肿瘤体积,达沙替尼+紫杉醇与紫杉醇:0.28 与 0.81 cm3,差异=0.53 cm3,95%置信区间[CI]为 0.44 至 0.62 cm3,P=0.014);达沙替尼+紫杉醇与达沙替尼:0.28 与 0.55 cm3,差异=0.27 cm3,95%CI 为 0.21 至 0.33 cm3,P=0.035)。联合治疗诱导的 TUNEL 阳性凋亡细胞多于单独使用任何一种药物。与阴性对照 siRNA 相比,p27(Kip1)的 siRNA 敲低降低了达沙替尼和紫杉醇诱导的细胞凋亡(亚 G1 期,对照 siRNA 与 p27(Kip1) siRNA:42.5%与 20.1%,差异=22.4%,95%CI 为 20.1%至 24.7%,P=0.017)。用强制表达和 Bcl-2 和 Cdk1 的 siRNA 研究表明,达沙替尼介导的 p27(Kip1)诱导通过负调节 Bcl-2 和 Cdk1 表达增强了紫杉醇诱导的细胞凋亡。
结论
用 siRNA 或达沙替尼抑制 Src 家族和 Abl 激酶通过 p27(Kip1)介导的 Bcl-2 和 Cdk1 表达抑制增强卵巢癌细胞对紫杉醇的敏感性。
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