El-Baba Chirine, Mahadevan Vijayalakshmi, Fahlbusch Fabian B, Mohan S Suma, Rau Tilman T, Gali-Muhtasib Hala, Schneider-Stock Regine
Experimental Tumorpathology, Institute of Pathology, Friedrich-Alexander University Erlangen-Nürnberg (FAU), Erlangen, Germany.
Mol Cancer. 2014 Aug 29;13:201. doi: 10.1186/1476-4598-13-201.
Thymoquinone (TQ) was shown to reduce tumor growth in several cancer models both in vitro and in vivo. So far only a few targets of TQ, including protein kinases have been identified. Considering that kinases are promising candidates for targeted anticancer therapy, we studied the complex kinase network regulated by TQ.
Novel kinase targets influenced by TQ were revealed by in silico analysis of peptide array data obtained from TQ-treated HCT116wt cells. Western blotting and kinase activity assays were used to determine changes in kinase expression patterns in colorectal cancer cells (HCT116wt, DLD-1, HT29). To study the viability/apoptotic effects of combining the PAK1 inhibitor IPA-3 and TQ, crystal violet assay and AnnexinV/PI staining were employed. Interactions between PAK1 and ERK1/2 were investigated by co-immunoprecipitation and modeled by docking studies. Transfection with different PAK1 mutants unraveled the role of TQ-induced changes in PAK1 phosphorylation and TQ's effects on PAK1 scaffold function.
Of the 104 proteins identified, 50 were upregulated ≥ 2 fold by TQ and included molecules in the AKT-MEK-ERK1/2 pathway. Oncogenic PAK1 emerged as an interesting TQ target. Time-dependent changes in two PAK1 phosphorylation sites generated a specific kinase profile with early increase in pPAK(Thr212) followed by late increase in pPAK(Thr423). TQ induced an increase of pERK1/2 and triggered the early formation of an ERK1/2-PAK1 complex. Modeling confirmed that TQ binds in the vicinity of Thr212 accompanied by conformational changes in ERK2-PAK1 binding. Transfecting the cells with the non-phosphorylatable mutant T212A revealed an increase of pPAK(Thr423) and enhanced apoptosis. Likewise, an increase in apoptosis was observed in cells transfected with both the kinase-dead K299R mutant and PAK1 siRNA. Using structural modeling we suggest that TQ interferes also with the kinase domain consequently disturbing its interaction with pPAK(Thr423), finally inhibiting MEK-ERK1/2 signaling and disrupting its prosurvival function. pERK1/2 loss was also validated in vivo.
Our study shows for the first time that the small molecule TQ directly binds to PAK1 changing its conformation and scaffold function. Because TQ affects the central RAF/MEK/ERK1/2 pathway, the combination of TQ with targeted therapies is worth considering for future anticancer treatments.
在多种癌症模型中,无论是体外还是体内实验,都已证明百里醌(TQ)可抑制肿瘤生长。到目前为止,仅确定了TQ的少数靶点,包括蛋白激酶。鉴于激酶是靶向抗癌治疗的有前景的候选靶点,我们研究了由TQ调节的复杂激酶网络。
通过对从TQ处理的HCT116wt细胞获得的肽阵列数据进行计算机分析,揭示受TQ影响的新型激酶靶点。使用蛋白质印迹法和激酶活性测定法来确定结肠癌细胞(HCT116wt、DLD-1、HT29)中激酶表达模式的变化。为了研究PAK1抑制剂IPA-3与TQ联合使用对细胞活力/凋亡的影响,采用了结晶紫测定法和AnnexinV/PI染色法。通过免疫共沉淀研究PAK1与ERK1/2之间的相互作用,并通过对接研究进行建模。用不同的PAK1突变体转染细胞,揭示了TQ诱导的PAK1磷酸化变化的作用以及TQ对PAK1支架功能的影响。
在鉴定出的104种蛋白质中,有50种被TQ上调≥2倍,包括AKT-MEK-ERK1/2途径中的分子。致癌性PAK1成为一个有趣的TQ靶点。两个PAK1磷酸化位点的时间依赖性变化产生了一种特定的激酶谱,pPAK(Thr212)早期增加,随后pPAK(Thr423)后期增加。TQ诱导pERK1/2增加,并触发ERK1/2-PAK1复合物的早期形成。建模证实TQ结合在Thr212附近,伴随着ERK2-PAK1结合的构象变化。用不可磷酸化的突变体T212A转染细胞,显示pPAK(Thr423)增加并增强了细胞凋亡。同样,在用激酶失活的K299R突变体和PAK1 siRNA转染的细胞中也观察到细胞凋亡增加。使用结构建模,我们认为TQ也干扰激酶结构域,从而扰乱其与pPAK(Thr423)的相互作用,最终抑制MEK-ERK1/2信号传导并破坏其促生存功能。pERK1/2的缺失在体内也得到了验证。
我们的研究首次表明,小分子TQ直接与PAK1结合,改变其构象和支架功能。由于TQ影响核心RAF/MEK/ERK1/2途径,TQ与靶向治疗联合用于未来的抗癌治疗值得考虑。
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