Abstract

Our preliminary studies of gene dosage abnormalities in ovarian cancer reveal numerous recurring abnormalities, many not previously known. WE BELIEVE THAT MANY OF THESE ABNORMALITIES REPRESENT GENETIC CHANGES THAT ENABLE TUMOR PROGRESSION AND THAT IDENTIFICATION OF THE INVOLVED GENES WILL LEAD TO IMPROVED DIAGNOSIS, PROGNOSIS AND THERAPY. The objectives of this proposal are to carefully map the regions of common abnormality, to investigate the role of these abnormalities in ovarian cancer progression and to begin the process of identifying the involved genes. We will accomplish these through the combined analysis of loss of heterozygosity (LOH), comparative genomic hybridization (CGH) and fluorescence in situ hybridization (FISH).
Our specific aims are to; 1. Precisely define regions of gene dosage abnormality in serous grade III tumors and explore the chromosomal events that are involved. The number of grade III tumors analyzed using CGH, FSH and LOH analyses of primary tumors will be increased to 100 in order to allow statistically precise characterization of abnormalities that occur at frequencies greater than 10% These combined data will be analyzed at each site of gene dosage abnormality to determine whether the abnormality occurred as a result of physical deletion, mitotic recombination, loss plus reduplication, development of aneuploidy, amplification, etc. In addition, FISH with probes to regions of amplification identified using CGH will be applied to metaphase spreads in short term cultures, when available, to determine whether amplification is extrachromosomal or intrachromosomal. We also will compare our CGH results with CGH measurements of 100 matched tumors made by Japanese collaborators in order to investigate possible ethnic or environmental differences between ovarian cancer in Japan and the United States. 2. Define the order in which gene dosage abnormalities occur during progression. Our preliminary analyses of ovarian cancers show that high grade tumors have accumulated numerous abnormalities, many highly correlated. We presume that these abnormalities contribute to progression and we will test the hypothesis that they occur more or less serially by analysis of 100 borderline + grade I tumors and 100 grade II tumors. We will explore the possibility that correlations between abnormalities provide additional information about athe nature of the progression process. 3. Begin analysis of how the gene dosage abnormalities influence biological and clinical behavior by identifying genes associated with regions of common gene dosage abnormality in order to understand their genetic nature and biological function. Work during this project period will focus on 3q26 and 16q and on genes under study in other projects in this Program Project. Specific genes to be studied include EGF, EGFR, TGFalpha, TGFbeta, VEGF, VEGFR, KGF, KGFR, HGF and HGFR.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Program Projects (P01)
Project #
3P01CA064602-04S1
Application #
6336421
Study Section
Project Start
1999-04-30
Project End
2001-01-31
Budget Start
1998-10-01
Budget End
1999-09-30
Support Year
4
Fiscal Year
2000
Total Cost
$230,600
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Type
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Lu, Z; Yang, H; Sutton, M N et al. (2014) ARHI (DIRAS3) induces autophagy in ovarian cancer cells by downregulating the epidermal growth factor receptor, inhibiting PI3K and Ras/MAP signaling and activating the FOXo3a-mediated induction of Rab7. Cell Death Differ 21:1275-89
Cheng, Kwai Wa; Agarwal, Roshan; Mitra, Shreya et al. (2012) Rab25 increases cellular ATP and glycogen stores protecting cancer cells from bioenergetic stress. EMBO Mol Med 4:125-41
Badgwell, D B; Lu, Z; Le, K et al. (2012) The tumor-suppressor gene ARHI (DIRAS3) suppresses ovarian cancer cell migration through inhibition of the Stat3 and FAK/Rho signaling pathways. Oncogene 31:68-79
Zou, Chun-Fang; Jia, Luoqi; Jin, Hongyan et al. (2011) Re-expression of ARHI (DIRAS3) induces autophagy in breast cancer cells and enhances the inhibitory effect of paclitaxel. BMC Cancer 11:22
Cheong, Jae-Ho; Park, Eun Sung; Liang, Jiyong et al. (2011) Dual inhibition of tumor energy pathway by 2-deoxyglucose and metformin is effective against a broad spectrum of preclinical cancer models. Mol Cancer Ther 10:2350-62
Agarwal, Roshan; Carey, Mark; Hennessy, Bryan et al. (2010) PI3K pathway-directed therapeutic strategies in cancer. Curr Opin Investig Drugs 11:615-28
Ishida, Seiko; McCormick, Frank; Smith-McCune, Karen et al. (2010) Enhancing tumor-specific uptake of the anticancer drug cisplatin with a copper chelator. Cancer Cell 17:574-83
Short, John D; Dere, Ruhee; Houston, Kevin D et al. (2010) AMPK-mediated phosphorylation of murine p27 at T197 promotes binding of 14-3-3 proteins and increases p27 stability. Mol Carcinog 49:429-39
Liu, Shuying; Murph, Mandi; Panupinthu, Nattapon et al. (2009) ATX-LPA receptor axis in inflammation and cancer. Cell Cycle 8:3695-701
Huang, Shaoyi; Chang, In Soon; Lin, Wenbo et al. (2009) ARHI (DIRAS3), an imprinted tumour suppressor gene, binds to importins and blocks nuclear import of cargo proteins. Biosci Rep 30:159-68

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