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Sp1对大鼠多聚(ADP-核糖)聚合酶基因的转录调控

Transcriptional regulation of the rat poly(ADP-ribose) polymerase gene by Sp1.

作者信息

Bergeron M J, Leclerc S, Laniel M A, Poirier G G, Guérin S L

机构信息

Laboratory of Molecular Endocrinology, CHUL Research Center, Ste-Foy, Qc, Canada.

出版信息

Eur J Biochem. 1997 Dec 1;250(2):342-53. doi: 10.1111/j.1432-1033.1997.0342a.x.

DOI:10.1111/j.1432-1033.1997.0342a.x
PMID:9428683
Abstract

Expression of the gene encoding poly(ADP-ribose) polymerase (PARP), although ubiquitous, nevertheless varies substantially between tissues. We have recently shown that Sp1 binds five distinct target sequences (US-1 and F1-F4) in the rat PARP (rPARP) gene promoter. Here we used deletion analyses and site-directed mutagenesis to address the regulatory function played by these Sp1 sites on the basal transcriptional activity directed by the rPARP promoter. Transfection experiments revealed that the most proximal Sp1 site is insufficient by itself to direct any promoter activity. In addition, a weak negative regulatory element was identified between positions -101 and -60. The rPARP promoter directed high levels of chloramphenicol acetyltransferase activity in Jurkat T-lymphoblastoid and Ltk- fibroblast cells but only moderate levels in pituitary GH4C1 and liver HTC cells, correlating with the amounts of PARP detected in these cells by western blot analysis. However, the reduced promoter efficiency in HTC and GH4C1 cells did not result from the lack of Sp1 activity in these cells but suggested that yet uncharacterized regulatory proteins might turn off PARP gene expression by binding negative regulatory elements from the rPARP promoter. Similarly, site-directed mutagenesis on the three most proximal Sp1 elements suggested the influence exerted by Sp1 on the rPARP promoter activity to vary substantially between cell types. It also provided evidence for a basal rPARP promoter activity driven through the recognition of unidentified cis-acting elements by transcription factors other than Sp1.

摘要

编码聚(ADP - 核糖)聚合酶(PARP)的基因表达虽然普遍存在,但在不同组织之间仍有很大差异。我们最近发现,Sp1结合大鼠PARP(rPARP)基因启动子中的五个不同靶序列(US - 1和F1 - F4)。在此,我们使用缺失分析和定点诱变来研究这些Sp1位点对rPARP启动子指导的基础转录活性所起的调节作用。转染实验表明,最靠近近端的Sp1位点本身不足以指导任何启动子活性。此外,在 - 101和 - 60位之间鉴定出一个弱负调控元件。rPARP启动子在Jurkat T淋巴母细胞和Ltk - 成纤维细胞中指导高水平的氯霉素乙酰转移酶活性,但在垂体GH4C1细胞和肝HTC细胞中仅指导中等水平的活性,这与通过蛋白质印迹分析在这些细胞中检测到的PARP量相关。然而,HTC和GH4C1细胞中启动子效率的降低并非由于这些细胞中Sp1活性的缺乏,而是表明尚未鉴定的调节蛋白可能通过结合rPARP启动子中的负调控元件来关闭PARP基因表达。同样,对三个最靠近近端的Sp1元件进行定点诱变表明,Sp1对rPARP启动子活性的影响在不同细胞类型之间有很大差异。这也为通过Sp1以外的转录因子识别未鉴定的顺式作用元件驱动的基础rPARP启动子活性提供了证据。

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