Biology Centre AS CR, v,v,i, AND University of South Bohemia, Branisovska 31, Ceske Budejovice, Czech Republic.
Breast Cancer Res. 2010;12(3):R30. doi: 10.1186/bcr2581. Epub 2010 May 27.
Breast cancer is one of the most common types of cancer in women. One of the genes that were found mutated in breast cancer is casein kinase 1 epsilon (CK1epsilon). Because CK1epsilon is a crucial regulator of the Wnt signaling cascades, we determined how these CK1epsilon mutations interfere with the Wnt pathway and affect the behavior of epithelial breast cancer cell lines.
We performed in silico modeling of various mutations and analyzed the kinase activity of the CK1epsilon mutants both in vitro and in vivo. Furthermore, we used reporter and small GTPase assays to identify how mutation of CK1epsilon affects different branches of the Wnt signaling pathway. Based on these results, we employed cell adhesion and cell migration assays in MCF7 cells to demonstrate a crucial role for CK1epsilon in these processes.
In silico modeling and in vivo data showed that autophosphorylation at Thr 44, a site adjacent to the breast cancer point mutations in the N-terminal lobe of human CK1epsilon, is involved in positive regulation of the CK1epsilon activity. Our data further demonstrate that, in mammalian cells, mutated forms of CK1epsilon failed to affect the intracellular localization and phosphorylation of Dvl2; we were able to demonstrate that CK1epsilon mutants were unable to enhance Dvl-induced TCF/LEF-mediated transcription, that CK1epsilon mutants acted as loss-of-function in the Wnt/beta-catenin pathway, and that CK1epsilon mutants activated the noncanonical Wnt/Rac-1 and NFAT pathways, similar to pharmacological inhibitors of CK1. In line with these findings, inhibition of CK1 promoted cell migration as well as decreased cell adhesion and E-cadherin expression in the breast cancer-derived cell line MCF7.
In summary, these data suggest that the mutations of CK1epsilon found in breast cancer can suppress Wnt/beta-catenin as well as promote the Wnt/Rac-1/JNK and Wnt/NFAT pathways, thus contributing to breast cancer development via effects on cell adhesion and migration. In terms of molecular mechanism, our data indicate that the breast cancer point mutations in the N-terminal lobe of CK1epsilon, which are correlated with decreased phosphorylation activities of mutated forms of CK1epsilon both in vitro and in vivo, interfere with positive autophosphorylation at Thr 44.
乳腺癌是女性最常见的癌症类型之一。在乳腺癌中发现的突变基因之一是酪蛋白激酶 1 ɛ(CK1ɛ)。由于 CK1ɛ 是 Wnt 信号级联的关键调节剂,我们确定了这些 CK1ɛ 突变如何干扰 Wnt 途径并影响上皮性乳腺癌细胞系的行为。
我们对各种突变进行了计算机建模,并在体外和体内分析了 CK1ɛ 突变体的激酶活性。此外,我们使用报告基因和小 GTPase 测定来确定 CK1ɛ 突变如何影响 Wnt 信号通路的不同分支。基于这些结果,我们在 MCF7 细胞中进行了细胞黏附和细胞迁移测定,以证明 CK1ɛ 在这些过程中的重要作用。
计算机建模和体内数据表明,Thr 44 处的自身磷酸化,该位点紧邻人 CK1ɛ N 端结构域中的乳腺癌点突变,参与 CK1ɛ 活性的正调节。我们的数据进一步表明,在哺乳动物细胞中,CK1ɛ 的突变形式未能影响 Dvl2 的细胞内定位和磷酸化;我们能够证明 CK1ɛ 突变体无法增强 Dvl 诱导的 TCF/LEF 介导的转录,CK1ɛ 突变体在 Wnt/β-catenin 途径中表现为功能丧失,并且 CK1ɛ 突变体激活非经典的 Wnt/Rac-1 和 NFAT 途径,类似于 CK1 的药理学抑制剂。与这些发现一致,CK1 的抑制促进了乳腺癌衍生细胞系 MCF7 中的细胞迁移以及细胞黏附和 E-钙黏蛋白表达的降低。
总之,这些数据表明,在乳腺癌中发现的 CK1ɛ 突变可以抑制 Wnt/β-catenin,同时促进 Wnt/Rac-1/JNK 和 Wnt/NFAT 途径,从而通过对细胞黏附和迁移的影响促进乳腺癌的发展。就分子机制而言,我们的数据表明,CK1ɛ N 端结构域中的乳腺癌点突变,其与体外和体内 CK1ɛ 突变体的磷酸化活性降低相关,干扰 Thr 44 处的正向自身磷酸化。
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