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三种检测方法均显示野生型和突变型 p53 与独特基因序列的结合存在差异。

Three assays show differences in binding of wild-type and mutant p53 to unique gene sequences.

机构信息

Department of Biological Sciences, Binghamton University, Binghamton, NY 13902, USA.

出版信息

Technol Cancer Res Treat. 2009 Dec;8(6):445-53. doi: 10.1177/153303460900800606.

Abstract

Cancer-associated mutations in the p53 gene often change amino acids in the protein's DNA binding domain. We used three different binding assays specifically gel shift, DNA binding scintillation proximity assay and a streptavidin magnetic bead assay to analyze the DNA binding of the tumor suppressor p53 from 4 human cell lines with different DNA sequences from the mdm2, p21 and cyclin G genes and a mutant form of the cyclin G sequence. Treatment of MCF-7 cells having wild-type p53 with hydrogen peroxide increased the binding of p53 to DNA as detected using all three assays, but to different extents. The p53 proteins from the thyroid cancer cell lines with different p53 mutations (ARO, WRO and NPA) have comparable binding reactions in the three assays, but show different specificities for the sequences. Here we show that multiple different binding assays allow us to generate a more complete picture of the function of DNA transcription factors in diseases such as cancer.

摘要

癌症相关的 p53 基因突变通常会改变蛋白质 DNA 结合域中的氨基酸。我们使用了三种不同的结合测定法,特别是凝胶迁移、DNA 结合闪烁接近测定法和链霉亲和素磁珠测定法,来分析来自 4 个人类细胞系的肿瘤抑制因子 p53 的 DNA 结合活性,这些细胞系的 DNA 序列与 mdm2、p21 和细胞周期蛋白 G 基因以及细胞周期蛋白 G 序列的突变体形式不同。用双氧水处理具有野生型 p53 的 MCF-7 细胞后,所有三种测定法均检测到 p53 与 DNA 的结合增加,但增加的程度不同。来自具有不同 p53 突变(ARO、WRO 和 NPA)的甲状腺癌细胞系的 p53 蛋白在三种测定法中具有相似的结合反应,但对序列的特异性不同。在这里,我们表明,多种不同的结合测定法使我们能够更全面地了解 DNA 转录因子在癌症等疾病中的功能。

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