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Identification of small molecule inhibitors of hypoxia- inducible factor 1 transcriptional activation pathway

  1. Author:
    Rapisarda, A.
    Uranchimeg, B.
    Scudiero, D. A.
    Selby, M.
    Sausville, E. A.
    Shoemaker, R. H.
    Melillo, G.

  2. Author Address

    NCI, DTP, Tumor Hypoxia Lab, Bldg 432,Room 218, Frederick, MD 21702 USA NCI, DTP, Tumor Hypoxia Lab, Frederick, MD 21702 USA NCI, Sci Applicat Int Corp, Frederick, MD 21702 USA Melillo G NCI, DTP, Tumor Hypoxia Lab, Bldg 432,Room 218, Frederick, MD 21702 USA
    1. Year: 2002
  2. Journal: Cancer Research
    1. 62
    2. 15
    3. Pages: 4316-4324
  4. Type of Article: Article
  1. Abstract:

    Hypoxia-inducible factor I (HIF-1) is a master regulator of the transcriptional response to oxygen deprivation. HIF-1 has been implicated in the regulation of genes involved in angiogenesis [e.g., vascular endothelial growth factor (VEGF) and inducible nitric oxide synthase] and anaerobic metabolism (e.g., glycolytic enzymes). HIF-1 is essential for angiogenesis and is associated with tumor progression. In addition, overexpression of HIF-1alpha has been demonstrated in many common human cancers. Therefore, HIF-1 is an attractive molecular target for development of novel cancer therapeutics. We have developed a cell-based high-throughput screen for the identification of small molecule inhibitors of the HIF-1 pathway. We have genetically engineered U251 human glioma cells to stably express a recombinant vector in which the luciferase reporter gene is under control of three copies of a canonical hypoxia- responsive element (U251-HRE). U251-HRE cells consistently expressed luciferase in a hypoxia- and HIF-1-dependent fashion. We now report the results of a pilot screen of the National Cancer Institute "Diversity Set," a collection of approximately 2000 compounds selected to represent the greater chemical diversity of the National Cancer Institute chemical repository. We found four compounds that specifically inhibited HIF-1- dependent induction of luciferase but not luciferase expression driven by a constitutive promoter. In addition, these compounds inhibited hypoxic induction of VEGF mRNA and protein expression in U251 cells. Interestingly, three compounds are closely related camptothecin analogues and topoisomerase (Topo)-I inhibitors. We show that concomitant with HIF-1 and VEGF inhibition, the activity of the Topo-I inhibitors tested is associated with induction of cyclooxygenase 2 mRNA expression. The luciferase-based high-throughput screen is a feasible tool for the identification of small molecule inhibitors of HIF-1 transcriptional activation. In addition, our results suggest that altered Topo-I function may be associated with repression of HIF-1-dependent induction of gene expression.

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