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p110 视网膜母细胞瘤蛋白的结合抑制猴病毒 SV40 大肿瘤抗原的核输入。

Binding of p110 retinoblastoma protein inhibits nuclear import of simian virus SV40 large tumor antigen.

机构信息

Nuclear Signaling Laboratory, Department of Biochemistry and Molecular Biology, Monash University, Victoria, Clayton 3800, Australia.

出版信息

J Biol Chem. 2010 Jun 4;285(23):17744-53. doi: 10.1074/jbc.M109.055491. Epub 2010 Mar 31.

Abstract

Nuclear import of the simian virus 40 large tumor antigen (T-ag) is dependent on its nuclear localization signal (NLS) within amino acids 126-132 that is recognized by the importin alpha/beta1 heterodimer, as well as a protein kinase CK2 site at serine 112 upstream of the NLS, which enhances the interaction approximately 50-fold. Here we show for the first time that T-ag nuclear import is negatively regulated by N-terminal sequences (amino acids 102-110), which represent the binding site (BS) for the retinoblastoma (Rb) tumor suppressor protein (p110(Rb)). Quantitative confocal laser scanning microscopic analysis of the transport properties of T-ag constructs with or without Rb binding site mutations in living transfected cells or in a reconstituted nuclear transport system indicates that the presence of the RbBS significantly reduces nuclear accumulation of T-ag. A number of approaches, including the analysis of T-ag nuclear import in an isogenic cell pair with and without functional p110(Rb) implicate p110(Rb) binding as being responsible for the reduced nuclear accumulation, with the Ser(106) phosphorylation site within the RbBS appearing to enhance the inhibitory effect. Immunoprecipitation experiments confirmed association of T-ag and p110(Rb) and dependence thereof on negative charge at Ser(106). The involvement of p110(Rb) in modulating T-ag nuclear transport has implications for the regulation of nuclear import of other proteins from viruses of medical significance that interact with p110(Rb), and how this may relate to transformation.

摘要

猿猴病毒 40 大肿瘤抗原(T-ag)的核输入依赖于其氨基酸 126-132 内的核定位信号(NLS),该信号被 importin alpha/beta1 异二聚体识别,以及 NLS 上游丝氨酸 112 处的蛋白激酶 CK2 位点,该位点增强了大约 50 倍的相互作用。在这里,我们首次表明 T-ag 核输入受到 N 端序列(氨基酸 102-110)的负调控,这些序列代表了视网膜母细胞瘤(Rb)肿瘤抑制蛋白(p110(Rb))的结合位点(BS)。活转染细胞或重建核转运系统中具有或不具有 Rb 结合位点突变的 T-ag 构建体的运输特性的定量共焦激光扫描显微镜分析表明,RbBS 的存在显着降低了 T-ag 的核积累。许多方法,包括在具有和不具有功能性 p110(Rb)的同基因细胞对中分析 T-ag 核输入,都表明 p110(Rb)结合是导致核积累减少的原因,而 RbBS 内的 Ser(106)磷酸化位点似乎增强了抑制作用。免疫沉淀实验证实了 T-ag 和 p110(Rb)的关联及其对 Ser(106)上负电荷的依赖性。p110(Rb)参与调节 T-ag 核转运对其他与 p110(Rb)相互作用的具有医学意义的病毒蛋白的核输入调节具有重要意义,以及这如何与转化相关。

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