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永生化PRKDC基因敲除细胞中癌基因Mdm2和孤儿受体基因Nr1h4的扩增与过表达。

Amplification and overexpression of oncogene Mdm2 and orphan receptor gene Nr1h4 in immortal PRKDC knockout cells.

作者信息

Ai Rong, Sandoval Ana, Chen David J, Burma Sandeep, Labhart Paul

机构信息

Torrey Pines Institute for Molecular Studies, 3550 General Atomics Court, San Diego, CA 92121, USA.

出版信息

Mol Biol Rep. 2004 Jun;31(2):91-6. doi: 10.1023/b:mole.0000031358.71141.78.

Abstract

DNA-dependent protein kinase (DNA-PK) is required for the repair of double strand DNA breaks by nonhomologous DNA end joining. The catalytic subunit of DNA-PK, PRKDC, may also be involved in repair-related or separate cell signaling pathways. To learn more about the cellular function of DNA-PK under normal physiological conditions, we identified genes that are differentially expressed between an immortalized wild-type mouse fibroblast cell line and its DNA-PK-deficient counterpart (Prkdc -/-). The proto-oncogene Mdm2 and the farnesoid X receptor gene Nrlh4 were overexpressed in the DNA-PK-deficient cell line. We show that in the DNA-PK-deficient cell line the genes for both Mdm2 and Nrlh4 are amplified to a degree that could account for most, if not all, of their increased expression. Other genes were strongly downregulated in the DNA-PK-deficient cell line, but this opposite expression pattern was not due to gene amplification in the wild-type cells. None of these genes was differentially expressed in DNA-PK-containing and DNA-PK-deficient primary mouse embryo fibroblasts. Our results suggest a model in which DNA-PK indirectly affects the cellular gene expression profile through its caretaker role and by preventing gene amplification.

摘要

DNA依赖性蛋白激酶(DNA-PK)是通过非同源DNA末端连接修复双链DNA断裂所必需的。DNA-PK的催化亚基PRKDC也可能参与与修复相关或独立的细胞信号通路。为了更多地了解DNA-PK在正常生理条件下的细胞功能,我们鉴定了在永生化野生型小鼠成纤维细胞系及其DNA-PK缺陷对应物(Prkdc-/-)之间差异表达的基因。原癌基因Mdm2和法尼醇X受体基因Nrlh4在DNA-PK缺陷细胞系中过表达。我们表明,在DNA-PK缺陷细胞系中,Mdm2和Nrlh4的基因均扩增到一定程度,这可以解释它们大部分(如果不是全部)表达增加的原因。其他基因在DNA-PK缺陷细胞系中强烈下调,但这种相反的表达模式并非由于野生型细胞中的基因扩增所致。这些基因在含有DNA-PK和缺乏DNA-PK的原代小鼠胚胎成纤维细胞中均无差异表达。我们的结果提出了一个模型,其中DNA-PK通过其守护者作用并通过防止基因扩增间接影响细胞基因表达谱。

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