Abstract

Cyclin E is a G I cyclin essential for S phase entry and has a profound role in oncogenesis. Previously this laboratory found that cyclin E is overexpressed and present in lower molecular weight (LMW) isoforms in breast cancer cells and tumor tissues compared to normal cells and tissues. Such alteration of cyclin E is linked to poor patient outcome. How cyclin E turns into these tumor specific LMW forms will be valuable in understanding the nature of the cell cycle disruption in the tumor phenotype. Our recent studies revealed that only tumor cells have the machinery to process cyclin E into its LMW forms. We have identified the region of cyclin E that is proteolytically cleaved to generate the LMW isoforms found in tumor cells through mutational and biochemical analysis. We were able to either generate or knockout the tumor specific LMW pattern of cyclin E by transient transfection of FLAG-tagged cyclin E constructs harboring specific mutations in a breast cancer cell line. These studies helped identify the putative site in the amino terminus of cyclin E targeted to generate these tumor specific LMW isoforms. This consensus sequence is targeted by a serine protease of the elastase class. We also show that not only are the LMW forms of cyclin E (2 examined so far) functional, as they phosphorylate substrates such as Histone Hi and GST-Rb, but their activities are higher than the full length cyclin E. Lastly, these nuclear localized LMW forms of cyclin E are biologically functional, as their overexpression in normal cells increases the ability of these cells to enter S and G2IM phase by 2 fold over vector alone transfected cells. These studies have raised the hypothesis that the defective entry into and exit from S phase by tumor cells is in part due to the loss of cyclin E regulation of the cell cycle; proteolytic processing of cyclin E results in LMW isoforms whose substrate selection has been modified from the full-length protein. The resulting deregulation of the cell cycle and altered substrate specificity of cyclin E contribute to the oncogenesis process. To test this hypothesis we will (a) identify all the LMW forms of cyclin E and examine their biochemical roles in vitro, (b) determine the biological, biochemical and oncological properties of the LMW forms of cyclin E in cultured cells and in vivo, (c) investigate the role of elastase in the processing of cyclin E into its LMW forms in tumor cells, and lastly, (d) examine the consequences of inhibition of elastases on cyclin E in human breast cancer cells. These studies are designed to understand the biochemical and cellular pathways through which the proteolytic processing of cyclin E leads to its oncogenic potential. This new understanding of tumor specific cyclin E deregulation may lead to development of novel prognostic markers and therapeutic targets for breast cancer-the second leading cause of cancer deaths of women in this country.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA087548-02
Application #
6522803
Study Section
Pathology B Study Section (PTHB)
Program Officer
Spalholz, Barbara A
Project Start
2001-08-01
Project End
2005-07-31
Budget Start
2002-08-01
Budget End
2003-07-31
Support Year
2
Fiscal Year
2002
Total Cost
$270,000
Indirect Cost

  Institution

Name
University of Texas MD Anderson Cancer Center
Department
Radiation-Diagnostic/Oncology
Type
Other Domestic Higher Education
DUNS #
001910777
City
Houston
State
TX
Country
United States
Zip Code
77030

  Publications

Caruso, Joseph A; Duong, Mylinh T; Carey, Jason P W et al. (2018) Low-Molecular-Weight Cyclin E in Human Cancer: Cellular Consequences and Opportunities for Targeted Therapies. Cancer Res 78:5481-5491
Carey, Jason P W; Karakas, Cansu; Bui, Tuyen et al. (2018) Synthetic Lethality of PARP Inhibitors in Combination with MYC Blockade Is Independent of BRCA Status in Triple-Negative Breast Cancer. Cancer Res 78:742-757
Chen, Xian; Low, Kwang-Huei; Alexander, Angela et al. (2018) Cyclin E Overexpression Sensitizes Triple-Negative Breast Cancer to Wee1 Kinase Inhibition. Clin Cancer Res 24:6594-6610
Doostan, Iman; Karakas, Cansu; Kohansal, Mehrnoosh et al. (2017) Cytoplasmic Cyclin E Mediates Resistance to Aromatase Inhibitors in Breast Cancer. Clin Cancer Res 23:7288-7300
Balaji, Kavitha; Vijayaraghavan, Smruthi; Diao, Lixia et al. (2017) AXL Inhibition Suppresses the DNA Damage Response and Sensitizes Cells to PARP Inhibition in Multiple Cancers. Mol Cancer Res 15:45-58
Vijayaraghavan, Smruthi; Karakas, Cansu; Doostan, Iman et al. (2017) CDK4/6 and autophagy inhibitors synergistically induce senescence in Rb positive cytoplasmic cyclin E negative cancers. Nat Commun 8:15916
Francis, Ashleigh M; Alexander, Angela; Liu, Yanna et al. (2017) CDK4/6 Inhibitors Sensitize Rb-positive Sarcoma Cells to Wee1 Kinase Inhibition through Reversible Cell-Cycle Arrest. Mol Cancer Ther 16:1751-1764
Hunt, Kelly K; Karakas, Cansu; Ha, Min Jin et al. (2017) Cytoplasmic Cyclin E Predicts Recurrence in Patients with Breast Cancer. Clin Cancer Res 23:2991-3002
Nanos-Webb, A; Bui, T; Karakas, C et al. (2016) PKCiota promotes ovarian tumor progression through deregulation of cyclin E. Oncogene 35:2428-40
Jabbour-Leung, Natalie A; Chen, Xian; Bui, Tuyen et al. (2016) Sequential Combination Therapy of CDK Inhibition and Doxorubicin Is Synthetically Lethal in p53-Mutant Triple-Negative Breast Cancer. Mol Cancer Ther 15:593-607

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