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6-磷酸果糖-2-激酶(pfkfb3)基因启动子包含缺氧诱导因子-1结合位点,这些位点是响应缺氧进行反式激活所必需的。

6-Phosphofructo-2-kinase (pfkfb3) gene promoter contains hypoxia-inducible factor-1 binding sites necessary for transactivation in response to hypoxia.

作者信息

Obach Mercè, Navarro-Sabaté Aurea, Caro Jaime, Kong Xianguo, Duran Joan, Gómez Marta, Perales Jose Carlos, Ventura Francesc, Rosa Jose Luis, Bartrons Ramon

机构信息

Unitat de Bioquímica i Biologia Molecular, Departament de Ciències Fisiològiques II, Campus de Bellvitge, Universitat de Barcelona, Feixa Llarga s/n, Pavelló de Govern, E-08907 L'Hospitalet, Spain.

出版信息

J Biol Chem. 2004 Dec 17;279(51):53562-70. doi: 10.1074/jbc.M406096200. Epub 2004 Oct 5.

DOI:10.1074/jbc.M406096200
PMID:15466858
Abstract

The up-regulation of glycolysis to enhance the production of energy under reduced pO(2) is a hallmark of the hypoxic response. A key regulator of glycolytic flux is fructose-2,6-bisphosphate, and its steady state concentration is regulated by the action of different isozymes product of four genes (pfkfb1-4). pfkfb3 has been found in proliferating cells and tumors, being induced by hypoxia. To understand the organization of cis-acting sequences that are responsible for the oxygen-regulated pfkfb3 gene, we have studied its 5'-flanking region. Extensive analysis of the 5' pfkfb3 promoter sequence revealed the presence of putative consensus binding sites for various transcription factors that could play an important role in pfkfb3 gene regulation. These DNA consensus sequences included estrogen receptor, hypoxia response element (HRE), early growth response, and specific protein 1 putative binding sites. Promoter deletion analysis as well as putative HREs sequences (wild type and mutated) fused to a c-fos minimal promoter unit constructs demonstrate that the sequence located from -1269 to -1297 relative to the start site is required for hypoxia-inducible factor 1 (HIF-1) induction. The effective binding of HIF-1 transcription factor to the HREs at -1279 and -1288 was corroborated by electrophoretic mobility shift assay and biotinylated oligonucleotide pull-down. In addition, HIF-1alpha null mouse embryo fibroblasts transfected with a full-length pfkfb3 promoter-luciferase reporter construct further demonstrated that HIF-1 protein was critically involved for hypoxia transactivation of this gene. Altogether, these results demonstrate that pfkfb3 is a hypoxia-inducible gene that is stimulated through HIF interaction with the consensus HRE site in its promoter region.

摘要

在低氧分压(pO₂)条件下上调糖酵解以增强能量产生是缺氧反应的一个标志。糖酵解通量的关键调节因子是果糖-2,6-二磷酸,其稳态浓度受四个基因(pfkfb1 - 4)不同同工酶产物的作用调节。pfkfb3已在增殖细胞和肿瘤中被发现,可被缺氧诱导。为了解负责氧调节的pfkfb3基因的顺式作用序列的组织情况,我们研究了其5'侧翼区域。对5' pfkfb3启动子序列的广泛分析揭示了各种转录因子的假定共有结合位点的存在,这些位点可能在pfkfb3基因调控中发挥重要作用。这些DNA共有序列包括雌激素受体、缺氧反应元件(HRE)、早期生长反应和特异性蛋白1假定结合位点。启动子缺失分析以及与c-fos最小启动子单元构建体融合的假定HRE序列(野生型和突变型)表明,相对于起始位点从-1269至-1297的序列是缺氧诱导因子1(HIF-1)诱导所必需的。电泳迁移率变动分析和生物素化寡核苷酸下拉实验证实了HIF-1转录因子与-1279和-1288处的HRE有效结合。此外,用全长pfkfb3启动子-荧光素酶报告构建体转染的HIF-1α基因敲除小鼠胚胎成纤维细胞进一步证明,HIF-1蛋白对于该基因的缺氧反式激活至关重要。总之,这些结果表明pfkfb3是一个缺氧诱导基因,通过HIF与其启动子区域的共有HRE位点相互作用而被激活。

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