疱疹病毒癌蛋白MEQ与细胞周期调节因子CDK2之间的功能相互作用。
Functional interactions between herpesvirus oncoprotein MEQ and cell cycle regulator CDK2.
作者信息
Liu J L, Ye Y, Qian Z, Qian Y, Templeton D J, Lee L F, Kung H J
机构信息
Department of Molecular Biology and Microbiology, School of Medicine, Case Western Reserve University, Cleveland, Ohio 44106, USA.
出版信息
J Virol. 1999 May;73(5):4208-19. doi: 10.1128/JVI.73.5.4208-4219.1999.
Marek's disease virus, an avian alphaherpesvirus, has been used as an excellent model to study herpesvirus oncogenesis. One of its potential oncogenes, MEQ, has been demonstrated to transform a rodent fibroblast cell line, Rat-2, in vitro by inducing morphological transformation and anchorage- and serum-independent growth and by protecting cells from apoptosis induced by tumor necrosis factor alpha, C2-ceramide, UV irradiation, or serum deprivation. In this report, we show that there is a cell cycle-dependent colocalization of MEQ protein and cyclin-dependent kinase 2 (CDK2) in coiled bodies and the nucleolar periphery during the G1/S boundary and early S phase. To our knowledge, this is the first demonstration that CDK2 is found to localize to coiled bodies. Such an in vivo association and possibly subsequent phosphorylation may result in the cytoplasmic translocation of MEQ protein. Indeed, MEQ is expressed in both the nucleus and the cytoplasm during the G1/S boundary and early S phase. In addition, we were able to show in vitro phosphorylation of MEQ by CDKs. We have mapped the CDK phosphorylation site of MEQ to be serine 42, a residue in the proximity of the bZIP domain. An indirect-immunofluorescence study of the MEQ S42D mutant, in which the CDK phosphorylation site was mutated to a charged residue, reveals more prominent cytoplasmic localization. This lends further support to the notion that the translocation of MEQ is regulated by phosphorylation. Furthermore, phosphorylation of MEQ by CDKs drastically reduces the DNA binding activity of MEQ, which may in part account for the lack of retention of MEQ oncoprotein in the nucleus. Interestingly, the localization of CDK2 in coiled bodies and the nucleolar periphery is observed only in MEQ-transformed Rat-2 cells, implicating MEQ in modifying the subcellular localization of CDK2. Taken together, our data suggest that there is a novel reciprocal modulation between the herpesvirus oncoprotein MEQ and CDK2.
马立克氏病病毒是一种禽α疱疹病毒,已被用作研究疱疹病毒致癌作用的优秀模型。其潜在致癌基因之一MEQ已被证明可在体外通过诱导形态转化、不依赖贴壁和血清生长以及保护细胞免受肿瘤坏死因子α、C2-神经酰胺、紫外线照射或血清剥夺诱导的凋亡,来转化啮齿动物成纤维细胞系Rat-2。在本报告中,我们表明在G1/S边界和S期早期,MEQ蛋白与细胞周期蛋白依赖性激酶2(CDK2)在卷曲小体和核仁周边存在细胞周期依赖性共定位。据我们所知,这是首次证明CDK2定位于卷曲小体。这种体内关联以及可能随后的磷酸化可能导致MEQ蛋白的细胞质转位。实际上,在G1/S边界和S期早期,MEQ在细胞核和细胞质中均有表达。此外,我们能够在体外证明CDK对MEQ的磷酸化作用。我们已将MEQ的CDK磷酸化位点定位为丝氨酸42,该残基靠近bZIP结构域。对MEQ S42D突变体(其中CDK磷酸化位点突变为带电荷残基)的间接免疫荧光研究显示,其细胞质定位更为明显。这进一步支持了MEQ的转位受磷酸化调节这一观点。此外,CDK对MEQ的磷酸化极大地降低了MEQ的DNA结合活性,这可能部分解释了MEQ癌蛋白在细胞核中缺乏保留的原因。有趣的是,仅在MEQ转化的Rat-2细胞中观察到CDK2在卷曲小体和核仁周边的定位,这表明MEQ参与了对CDK2亚细胞定位的修饰。综上所述,我们的数据表明疱疹病毒癌蛋白MEQ与CDK2之间存在一种新的相互调节关系。
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