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中间丝的调节机制与功能:一项使用位点和磷酸化状态特异性抗体的研究。

Regulatory mechanisms and functions of intermediate filaments: a study using site- and phosphorylation state-specific antibodies.

作者信息

Izawa Ichiro, Inagaki Masaki

机构信息

Division of Biochemistry, Aichi Cancer Center Research Institute, Nagoya 464-8681, Japan.

出版信息

Cancer Sci. 2006 Mar;97(3):167-74. doi: 10.1111/j.1349-7006.2006.00161.x.

Abstract

Intermediate filaments (IF) form the structural framework of the cytoskeleton. Although histopathological detection of IF proteins is utilized for examining cancer specimens as reliable markers, the molecular mechanisms by which IF are involved in the biology of cancer cells are still unclear. We found that site-specific phosphorylation of IF proteins induces the disassembly of filament structures. To further dissect the in vivo spatiotemporal dynamics of IF phosphorylation, we developed site- and phosphorylation state-specific antibodies. Using these antibodies, we detected kinase activities that specifically phosphorylate type III IF, including vimentin, glial fibrillary acidic protein and desmin, during mitosis. Cdk1 phosphorylates vimentin-Ser55 from prometaphase to metaphase, leading to the recruitment of Polo-like kinase 1 (Plk1) to vimentin. Upon binding to Phospho-Ser55 of vimentin, Plk1 is activated, and then phosphorylates vimentin-Ser82. During cytokinesis, Rho-kinase and Aurora-B specifically phosphorylate IF at the cleavage furrow. IF phosphorylation by Cdk1, Plk1, Rho-kinase and Aurora-B plays an important role in the local IF breakdown, and is essential for the efficient segregation of IF networks into daughter cells. As another part of our research on IF, we have set out to find the binding partners with simple epithelial keratin 8/18. We identified tumor necrosis factor receptor type 1-associated death domain protein (TRADD) as a keratin 18-binding protein. Together with data from other laboratories, it is proposed that simple epithelial keratins may play a role in modulating the response to some apoptotic signals. Elucidation of the precise molecular functions of IF is expected to improve our understanding of tumor development, invasion and metastasis.

摘要

中间丝(IF)构成细胞骨架的结构框架。尽管IF蛋白的组织病理学检测被用作检查癌症标本的可靠标志物,但IF参与癌细胞生物学过程的分子机制仍不清楚。我们发现IF蛋白的位点特异性磷酸化会诱导丝状结构的解体。为了进一步剖析IF磷酸化在体内的时空动态,我们开发了位点和磷酸化状态特异性抗体。使用这些抗体,我们检测到在有丝分裂期间特异性磷酸化III型IF(包括波形蛋白、胶质纤维酸性蛋白和结蛋白)的激酶活性。细胞周期蛋白依赖性激酶1(Cdk1)在前期到中期磷酸化波形蛋白的Ser55,导致Polo样激酶1(Plk1)募集到波形蛋白上。与波形蛋白的磷酸化Ser55结合后,Plk1被激活,然后磷酸化波形蛋白的Ser82。在胞质分裂期间,Rho激酶和极光激酶B在分裂沟处特异性磷酸化IF。Cdk1、Plk1、Rho激酶和极光激酶B介导的IF磷酸化在局部IF解体中起重要作用,并且对于IF网络有效分离到子细胞中至关重要。作为我们对IF研究的另一部分,我们已着手寻找与简单上皮角蛋白8/18结合的伙伴。我们鉴定出肿瘤坏死因子受体1相关死亡结构域蛋白(TRADD)为角蛋白18结合蛋白。结合其他实验室的数据,有人提出简单上皮角蛋白可能在调节对某些凋亡信号的反应中发挥作用。对IF精确分子功能的阐明有望增进我们对肿瘤发生、侵袭和转移的理解。

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