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Increased AP-1 activity in drug resistant human breast cancer MCF-7 cells

  1. Author:
    Daschner, P. J.
    Ciolino, H. P.
    Plouzek, C. A.
    Yeh, G. C.

  2. Author Address

    Yeh GC NCI, Cellular Def & Carcinogenesis Sect, Basic Res Lab, FCRDC,NIH Bldg 560,Rm 12-91 Frederick, MD 21702 USA NCI, Cellular Def & Carcinogenesis Sect, Basic Res Lab, FCRDC,NIH Frederick, MD 21702 USA NCI, Intramural Res Support Program, SAIC, FCRDC Frederick, MD 21702 USA
    1. Year: 1999
  2. Journal: Breast Cancer Research and Treatment
    1. 53
    2. 3
    3. Pages: 229-240
  4. Type of Article: Article
  1. Abstract:

    The expression, DNA binding, and transactivating activity of activator protein 1 (AP-1) was examined in a series of multidrug resistant (MDR) MCF-7 human breast cancer cells that have increasing levels of MDR1 gene expression. We observed an increase in the amount of both c-jun and c-fos mRNA in cells with 12-, 65-, or 200-fold higher resistance to adriamycin when compared to drug-sensitive MCF-7 wild type (WT) cells. Electrophoretic mobility shift assays (EMSA) demonstrated an increase in the DNA binding activity of an AP-1 complex in nuclear extracts from MDR MCF-7 cells when compared to extracts from WT cells. We observed a proportional increase in luciferase expression from a reporter vector containing consensus AP-1 binding sites in transiently transfected MDR cells when compared to WT cells, indicating that AP-1 mediated gene expression is increased in drug-resistant MCF-7 cells. Since the MDR1 promoter contains a putative AP-1 binding site, we used EMSA to examine AP-1 binding activity to an oligonucleotide probe that contained the relevant MDR1 promoter sequences (-123 to -108). Nuclear extracts from resistant MCF-7 cells displayed an increased level of DNA binding of Jun/Jun dimers to the probe, indicating that AP-1 was capable of binding to this promoter site. A luciferase reporter construct containing triplicate copies of the MDR1 promoter sequence was expressed at higher levels in transiently transfected MDR cells when compared to expression in WT cells. Co-transfection of WT cells with a c-jun expression vector and either of the AP-1 luciferase constructs demonstrated that c-jun could activate gene expression from both the consensus and the MDR1 AP-1 sites in a dose dependent manner. In addition, RT-PCR and western blot analysis showed that levels of MDR1 mRNA and Pgp were increased in c-jun transfected WT cells. Taken together, these data indicate that increased AP-1 activity may be an important mediator of MDR by regulating the expression of MDR1. [References: 57]

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