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人增殖细胞核抗原(PCNA)基因座上两个不同启动子的体内结构。内含子1中反义RNA的合成及E2F复合物的S期依赖性结合。

In vivo structure of two divergent promoters at the human PCNA locus. Synthesis of antisense RNA and S phase-dependent binding of E2F complexes in intron 1.

作者信息

Tommasi S, Pfeifer G P

机构信息

Department of Biology, Beckman Research Institute, City of Hope National Medical Center, Duarte, California 91010, USA.

出版信息

J Biol Chem. 1999 Sep 24;274(39):27829-38. doi: 10.1074/jbc.274.39.27829.

DOI:10.1074/jbc.274.39.27829
PMID:10488129
Abstract

Proliferating cell nuclear antigen (PCNA) synthesis is strictly regulated during the cell cycle. To investigate PCNA transcriptional regulation, we have analyzed protein-DNA interactions at the promoter region and in the first intron in quiescent fibroblasts and following serum stimulation. Twenty putative protein-binding sites, distributed in two divergent promoters at the PCNA locus, were identified in vivo by genomic footprinting. These elements bind transcription factors continuously throughout the cell cycle with the exception of one E2F consensus site, located in the first intron at position +583. This E2F site becomes strongly occupied 18 h after serum stimulation, implying that an E2F activator complex plays a role in activation of the PCNA gene at the onset of S phase. We detected a 500-600-base pair-long antisense transcript by Northern blot analysis. This RNA has no apparent coding capacity and is constitutively transcribed from a promoter located within the first intron. We suggest that silencing of the PCNA gene is accomplished through base pairing between sense pre-mRNA and antisense RNA. The binding of S phase-specific E2F complexes at the +583 element may help to overcome the negative effect of the antisense transcript, which results in up-regulation of PCNA expression in proliferating cells.

摘要

增殖细胞核抗原(PCNA)的合成在细胞周期中受到严格调控。为了研究PCNA的转录调控,我们分析了静止成纤维细胞以及血清刺激后,启动子区域和第一个内含子中的蛋白质-DNA相互作用。通过基因组足迹法在体内鉴定出了20个推定的蛋白质结合位点,它们分布在PCNA基因座的两个不同启动子中。除了位于第一个内含子中+583位置的一个E2F共有位点外,这些元件在整个细胞周期中持续结合转录因子。血清刺激18小时后,这个E2F位点被强烈占据,这意味着一个E2F激活复合物在S期开始时对PCNA基因的激活中发挥作用。通过Northern印迹分析,我们检测到了一个500 - 600个碱基对长的反义转录本。该RNA没有明显的编码能力,由位于第一个内含子内的启动子组成型转录。我们认为PCNA基因的沉默是通过有义前体mRNA与反义RNA之间的碱基配对实现的。S期特异性E2F复合物在+583元件处的结合可能有助于克服反义转录本的负面影响,从而导致增殖细胞中PCNA表达上调。

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