Zhang Xue, Zhang Yun-wu, Liu Shijie, Bulloj Ayelen, Tong Gary G, Zhang Zhuohua, Liao Francesca-Fang, Xu Huaxi
Center for Neuroscience and Aging, Burnham Institute for Medical Research, 10901 N, Torrey Pines Road, La Jolla, CA 92037, USA.
Mol Neurodegener. 2006 Jul 31;1:7. doi: 10.1186/1750-1326-1-7.
Aberrant hyperphosphorylation of tau protein has been implicated in a variety of neurodegenerative disorders. Although a number of protein kinases have been shown to phosphorylate tau in vitro and in vivo, the molecular mechanisms by which tau phosphorylation is regulated pathophysiologically are largely unknown. Recently, a growing body of evidence suggests a link between tau phosphorylation and PI3K signaling. In this study, phosphorylation, aggregation and binding to the microtubule of a mutant frontal temporal dementia and parkinsonism linked to chromosome 17 (FTDP-17) tau in the presence of tumor suppressor PTEN, a major regulatory component in PI3K signaling, were investigated.
Phosphorylation of the human mutant FTDP-17 tau, T40RW, was evaluated using different phospho-tau specific antibodies in the presence of human wild-type or phosphatase activity null mutant PTEN. Among the evaluated phosphorylation sites, the levels of Ser214 and Thr212 phospho-tau proteins were significantly decreased in the presence of wild-type PTEN, and significantly increased when the phosphatase activity null mutant PTEN was ectopically expressed. Fractionation of the mutant tau transfected cells revealed a significantly increased level of soluble tau in cytosol when wild-type PTEN was expressed, and an elevated level of SDS-soluble tau aggregates in the presence of the mutant PTEN. In addition, the filter/trap assays detected more SDS-insoluble mutant tau aggregates in the cells overexpressing the mutant PTEN compared to those in the cells overexpressing wild-type PTEN and control DNA. This notion was confirmed by the immunocytochemical experiment which demonstrated that the overexpression of the phosphatase activity null mutant PTEN caused the mutant tau to form aggregates in the COS-7 cells.
Tumor suppressor PTEN can alleviate the phosphorylation of the mutant FTDP-17 tau at specific sites, and the phosphatase activity null PTEN increases the mutant tau phosphorylation at these sites. The changes of the tau phosphorylation status by ectopic expression of PTEN correlate to the alteration of the mutant tau's cellular distribution. In addition, the overexpression of the mutant PTEN can increase the level of the mutant tau aggregates and lead to the formation of visible aggregates in the cells.
tau蛋白的异常过度磷酸化与多种神经退行性疾病有关。尽管已证实在体外和体内有多种蛋白激酶可使tau磷酸化,但tau磷酸化在病理生理过程中被调控的分子机制却 largely 未知。最近,越来越多的证据表明tau磷酸化与PI3K信号传导之间存在联系。在本研究中,研究了在肿瘤抑制因子PTEN(PI3K信号传导中的主要调节成分)存在的情况下,与17号染色体相关的突变型额颞叶痴呆和帕金森综合征(FTDP - 17)tau蛋白的磷酸化、聚集以及与微管的结合情况。
在人野生型或磷酸酶活性缺失突变型PTEN存在的情况下,使用不同的磷酸化tau特异性抗体评估了人突变型FTDP - 17 tau(T40RW)的磷酸化情况。在评估的磷酸化位点中,野生型PTEN存在时,Ser214和Thr212磷酸化tau蛋白水平显著降低,而当磷酸酶活性缺失突变型PTEN异位表达时则显著升高。对转染了突变型tau的细胞进行分级分离发现,表达野生型PTEN时,胞质溶胶中可溶性tau水平显著升高,而在突变型PTEN存在时,SDS可溶性tau聚集体水平升高。此外,滤膜/捕获分析检测到,与过表达野生型PTEN和对照DNA的细胞相比,过表达突变型PTEN的细胞中SDS不溶性突变型tau聚集体更多。免疫细胞化学实验证实了这一观点,该实验表明磷酸酶活性缺失突变型PTEN的过表达导致突变型tau在COS - 7细胞中形成聚集体。
肿瘤抑制因子PTEN可减轻突变型FTDP - 17 tau在特定位点的磷酸化,而磷酸酶活性缺失的PTEN会增加这些位点的突变型tau磷酸化。通过PTEN异位表达引起的tau磷酸化状态变化与突变型tau细胞分布的改变相关。此外,突变型PTEN的过表达可增加突变型tau聚集体水平,并导致细胞中形成可见聚集体。
Zotero 插件
