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肿瘤抑制蛋白p53对纤溶酶原激活物抑制剂-1表达的调控

Regulation of plasminogen activator inhibitor-1 expression by tumor suppressor protein p53.

作者信息

Shetty Sreerama, Shetty Praveenkumar, Idell Steven, Velusamy Thirunavukkarasu, Bhandary Yashodhar P, Shetty Rashmi S

机构信息

Texas Lung Injury Institute, University of Texas Health Center, Tyler, Texas 75708, USA.

出版信息

J Biol Chem. 2008 Jul 11;283(28):19570-80. doi: 10.1074/jbc.M710268200. Epub 2008 May 9.

Abstract

H1299 lung carcinoma cells lacking p53 (p53-/-) express minimal amounts of plasminogen activator inhibitor-1 (PAI-1) protein as well as mRNA. p53(-/-) cells express highly unstable PAI-1 mRNA. Transfection of p53 in p53(-/-) cells enhanced PAI-1 expression and stabilized PAI-1 mRNA. On the contrary, inhibition of p53 expression by RNA silencing in non-malignant human lung epithelial (Beas2B) cells decreased basal as well as urokinase-type plasminogen activator-induced PAI-1 expression because of accelerated degradation of PAI-1 mRNA. Purified p53 protein specifically binds to the PAI-1 mRNA 3'-un-translated region (UTR), and endogenous PAI-1 mRNA forms an immune complex with p53. Treatment of purified p53 protein with anti-p53 antibody abolished p53 binding to the 3'-UTR of PAI-1 mRNA. The p53 binding region maps to a 70-nucleotide PAI-1 mRNA 3'-UTR sequence, and insertion of the p53-binding sequence into beta-globin mRNA destabilized the chimeric transcript. Deletion experiments indicate that the carboxyl-terminal region (amino acid residues 296-393) of p53 protein interacts with PAI-1 mRNA. These observations demonstrate a novel role for p53 as an mRNA-binding protein that regulates increased PAI-1 expression and stabilization of PAI-1 mRNA in human lung epithelial and carcinoma cells.

摘要

缺乏p53(p53-/-)的H1299肺癌细胞表达极少量的纤溶酶原激活物抑制剂-1(PAI-1)蛋白和mRNA。p53(-/-)细胞表达高度不稳定的PAI-1 mRNA。在p53(-/-)细胞中转染p53可增强PAI-1表达并稳定PAI-1 mRNA。相反,在非恶性人肺上皮(Beas2B)细胞中通过RNA沉默抑制p53表达,由于PAI-1 mRNA加速降解,降低了基础以及尿激酶型纤溶酶原激活物诱导的PAI-1表达。纯化的p53蛋白特异性结合PAI-1 mRNA的3'-非翻译区(UTR),内源性PAI-1 mRNA与p53形成免疫复合物。用抗p53抗体处理纯化的p53蛋白可消除p53与PAI-1 mRNA 3'-UTR的结合。p53结合区域定位于70个核苷酸的PAI-1 mRNA 3'-UTR序列,将p53结合序列插入β-珠蛋白mRNA会使嵌合转录本不稳定。缺失实验表明p53蛋白的羧基末端区域(氨基酸残基296-393)与PAI-1 mRNA相互作用。这些观察结果证明了p53作为一种mRNA结合蛋白的新作用,它在人肺上皮细胞和癌细胞中调节PAI-1表达增加和PAI-1 mRNA的稳定。

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