TNK2可维持表皮生长因子受体在细胞表面的表达,并增强人乳腺癌细胞的迁移和侵袭能力。
TNK2 preserves epidermal growth factor receptor expression on the cell surface and enhances migration and invasion of human breast cancer cells.
作者信息
Howlin Jillian, Rosenkvist Jeanette, Andersson Tommy
机构信息
Cell and Experimental Pathology, Lund University, Department of Laboratory Medicine, Clinical Research Centre, Ent 72, Bldg 91, fl 11, Malmö University Hospital, S-205 02 Malmö, Sweden.
出版信息
Breast Cancer Res. 2008;10(2):R36. doi: 10.1186/bcr2087. Epub 2008 Apr 24.
INTRODUCTION
Amplification of the TNK2 gene in primary tumours correlates with poor prognosis. In accordance, TNK2 overexpression was shown to promote invasion of cancer cells--but the mechanism by which TNK2 mediates these effects is unresolved. TNK2 was suggested to regulate Cdc42-driven migration by activation of breast cancer antioestrogen resistance 1 (BCAR1); however, distinct from this effect is evidence for a role of TNK2 in the regulation of epidermal growth factor receptor (EGFR) endocytosis and degradation. In the present study we sought to investigate whether negative targeting of TNK2 by siRNA could be used to inhibit cancer cell invasion, to establish the contribution of its effect on the EGFR and to consequently attempt to resolve the issue of TNK2's mechanism of action.
METHODS
We used siRNA to knockdown expression of TNK2 and its proposed effector BCAR1 in order to analyse the effect of this knockdown on cancer cell behaviour in vitro. We examined morphological changes using phase-contrast microscopy and immunohistochemistry. Functional parameters examined included apoptosis, proliferation, migration and invasion. We also performed flow cytometry analysis to examine EGFR cell surface expression and carried out western blot to examine the total EGFR levels.
RESULTS
We observed that targeting of TNK2 by siRNA in breast cancer cells resulted in distinct morphological changes characterised by a stellate appearance and an absence of protrusions at membrane edges. These changes were not recapitulated upon siRNA targeting of BCAR1. We thus hypothesised that a component of the effects induced by TNK2 may be independent of BCAR1. Consistent with the idea of an alternative mechanism for TNK2, we observed that TNK2 associates with activated EGFR in breast cancer cells in a TNK2-kinase-independent manner. Furthermore, we demonstrated that TNK2 functions to maintain EGFRs on the cell surface. We could demonstrate that the main functional effect of activating these surface EGFRs in breast cancer cells is stimulation of migration. In accordance, TNK2 silencing by siRNA led to a significant reduction in cell surface EGFR and to a concomitant decrease in the migratory and invasive capacity of breast cancer cells.
CONCLUSION
Our data suggest that TNK2 can enhance migration and invasion of breast cancer cells via preservation of EGFR expression, notwithstanding its previously reported signalling via BCAR1, explaining its oncogenic behaviour in vitro and correlation with metastatic human breast cancer in vivo.
引言
原发性肿瘤中TNK2基因的扩增与预后不良相关。相应地,TNK2的过表达被证明可促进癌细胞的侵袭——但TNK2介导这些效应的机制尚未明确。有人提出TNK2通过激活乳腺癌抗雌激素耐药蛋白1(BCAR1)来调节由Cdc42驱动的迁移;然而,与这种效应不同的是,有证据表明TNK2在表皮生长因子受体(EGFR)的内吞作用和降解调节中发挥作用。在本研究中,我们试图探究通过小干扰RNA(siRNA)对TNK2进行负向靶向是否可用于抑制癌细胞侵袭,确定其对EGFR的作用机制,并进而尝试解决TNK2作用机制的问题。
方法
我们使用siRNA敲低TNK2及其推测的效应分子BCAR1的表达,以分析这种敲低对体外癌细胞行为的影响。我们使用相差显微镜和免疫组织化学检查形态学变化。检测的功能参数包括细胞凋亡、增殖、迁移和侵袭。我们还进行了流式细胞术分析以检测EGFR的细胞表面表达,并进行蛋白质印迹法检测总EGFR水平。
结果
我们观察到,在乳腺癌细胞中用siRNA靶向TNK2会导致明显的形态学变化,其特征为星状外观且膜边缘无突起。在对BCAR1进行siRNA靶向时未出现这些变化。因此我们推测,TNK2诱导的效应的一部分可能独立于BCAR1。与TNK2存在另一种作用机制的观点一致,我们观察到TNK2以不依赖TNK2激酶的方式与乳腺癌细胞中激活的EGFR结合。此外,我们证明TNK2的功能是维持细胞表面的EGFR。我们能够证明,在乳腺癌细胞中激活这些表面EGFR的主要功能效应是刺激迁移。相应地,用siRNA沉默TNK2会导致细胞表面EGFR显著减少,并伴随乳腺癌细胞迁移和侵袭能力的降低。
结论
我们的数据表明,TNK2可通过维持EGFR表达来增强乳腺癌细胞的迁移和侵袭能力,尽管其先前报道的通过BCAR1的信号传导,这解释了其在体外的致癌行为以及与体内转移性人类乳腺癌的相关性。
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