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p53核输入的遗传分析

Genetic analysis of p53 nuclear importation.

作者信息

Li Q, Falsey R R, Gaitonde S, Sotello V, Kislin K, Martinez J D

机构信息

Department of Cell Biology and Anatomy, Arizona Cancer Center, University of Arizona, Tucson, AZ 85724, USA.

出版信息

Oncogene. 2007 Dec 13;26(57):7885-93. doi: 10.1038/sj.onc.1210597. Epub 2007 Jun 18.

Abstract

A key step in activation of the p53 tumor suppressor is its transport into the nucleus; however, despite intensive study of p53, the regulation of its subcellular localization is still poorly understood. Here we examined the p53 nuclear importation using a series of mutant cell lines that were resistant to the growth inhibitory effects of temperature-sensitive murine p53 (tsp53). Examination of the p53 subcellular localization in these cell lines showed that the protein was cytoplasmic in most of them. Using a digitonin-permeabilized cell in vitro nuclear import system, we show that cytosols from these cell lines do not support nuclear translocation of a p53 nuclear localization signal (NLS)-containing substrate protein, but promote nuclear localization of a SV40TAgNLS-containing substrate. Complementation assays and use of the mutant cells themselves in the in vitro assays demonstrate that both soluble and insoluble protein components are involved in p53 nuclear import. Collectively, our results suggest that there is a p53 NLS-selective nuclear import pathway and that both soluble and insoluble proteins are involved in its function.

摘要

p53肿瘤抑制因子激活过程中的关键一步是其转运至细胞核;然而,尽管对p53进行了深入研究,但其亚细胞定位的调控仍知之甚少。在此,我们使用了一系列对温度敏感型小鼠p53(tsp53)的生长抑制作用具有抗性的突变细胞系,研究了p53的核输入。对这些细胞系中p53的亚细胞定位进行检测,结果显示大多数细胞系中的该蛋白位于细胞质中。利用洋地黄皂苷通透细胞体外核输入系统,我们发现这些细胞系的胞质溶胶不支持含p53核定位信号(NLS)的底物蛋白的核转位,但能促进含SV40TAgNLS的底物的核定位。互补试验以及在体外试验中使用突变细胞本身表明,可溶性和不溶性蛋白成分均参与p53的核输入。总体而言,我们的结果表明存在一条p53 NLS选择性核输入途径,且可溶性和不溶性蛋白均参与其功能。

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