The long time goals of this project are to understand, in molecular terms, how signaling networks regulate the cellular response to DNA damage. Cellular DNA must be accurately replicated and transmitted to each daughter cell during cell division. In response to various forms of genotoxic stress, cells activate complex protein kinase signaling pathways, such as ATM, to arrest the cell cycle, recruit DNA repair machinery, and re-enter the cell cycle once the damage is resolved, or if the damage is overwhelming, induce apoptosis or cell senescence. In the present proposal, we explore the function of BAAT1, an activator of ATM under conditions of cell stress, as a critical regulator of DNA damage-sensing pathway in response to environmental and endogenous types of DNA damage. We use a combination of extensive biochemistry and molecular cell biology to explore the signal transduction mechanisms involved in BAAT1/ATM activation after DNA damage induced by ionizing radiation (IR) and chemicals, and examine how BAAT1/ATM pathway functions together with other checkpoint proteins such as NBS1, to control cell cycle progression after genotoxic stress in cells in culture. We go on to develop a conditional BAAT1 knockout mouse to explore whether BAAT1 functions in tumor suppressor pathway in genetically defined models of breast cancer, and in environmental carcinogen-induced models of colorectal cancer. Finally, we explore whether down-regulation of BAAT1 facilitates cell death after intentional chemically-induced DNA damage such as chemotherapy. These studies should clarify how signals from ATM pathway, a global stress- responsive network that is activated by a wide variety of toxic insults, integrate with those from dedicated DNA damage response pathways, to regulate the cellular response to genotoxic stress. The results of the proposed experiments should reveal whether BAAT1 functions as a tumor suppressor gene that modulates the risk of cancer after exposure to environmental agents, and whether specific targeting of BAAT1/ATM would be of therapeutic value for sensitizing tumors to the cytotoxic effects of conventional chemotherapy.

Public Health Relevance

The long time goals of this project are to understand, in molecular terms, how signaling networks regulate the cellular response to DNA damage. Cellular DNA must be accurately replicated and transmitted to each daughter cell during cell division. In response to various forms of genotoxic stress, cells activate complex protein kinase signaling pathways to arrest the cell cycle, recruit DNA repair machinery, and re-enter the cell cycle once the damage is resolved, or if the damage is overwhelming, induce apoptosis or cell senescence. DNA lesions arise as a consequence of both endogenous cellular processes such as metabolic reactions and DNA replication, and through exposure of cells to environmental mutagens including chemical carcinogens, UV light and gamma-radiation. A variety of incompletely understood genetic factors increase the risk for, and consequences of, DNA damage, and cell cycle control. Two canonical protein kinase pathways are responsible for arresting the cell cycle in response to damaged DNA - the ATR-Chk1 pathway and the ATM-Chk2 pathway. Disruption of either pathway is associated with increased sensitivity of cells to various DNA damaging agents, as well as with increase risk of various human cancers. We recently identified a protein, termed BAAT1 (BRCA1 Associated protein required for ATM activation-1). Biochemical studies have demonstrated that BAAT1 is required for autophosphorylation of ATM Ser1981, which has been shown to be essential for the activation of ATM under conditions of genotoxic stresses. Importantly, it has been revealed that the ATM pathway is a much more global stress-sensing pathway, and can be activated by different types of cellular stress including gamma-radiation, NaCl, chloroquine and Trichostatin A. We therefore hypothesize that the proper cellular response to genotoxic stress must involve the functional integration of dedicated DNA damage response pathways with stress kinase signaling pathways. In this proposal we seek to clarify how the BAAT1-ATM pathway is activated in response to DNA damage, how the BAAT1-ATM pathway is functionally interconnected with other DNA damage-sensing proteins, and whether cell specific-disruption of the BAAT1 pathway using RNA gene targeting approaches facilitates tumor development by genetic and environmental lesions or alters the response to tumors to DNA damaging chemotherapy.

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project--Cooperative Agreements (U01)
Project #
7U01CA090631-10
Application #
8399339
Study Section
Cancer Etiology Study Section (CE)
Program Officer
Pelroy, Richard
Project Start
2001-04-01
Project End
2013-05-31
Budget Start
2011-10-25
Budget End
2012-05-31
Support Year
10
Fiscal Year
2011
Total Cost
$268,065
Indirect Cost
Name
Roswell Park Cancer Institute Corp
Department
Type
DUNS #
824771034
City
Buffalo
State
NY
Country
United States
Zip Code
14263
So, Eui Young; Kozicki, Martin; Ouchi, Toru (2013) Roles of DNA Damage Response Proteins in Mitogen-Induced Thp-1 Differentiation into Macrophage. J Cancer Biol Res 1:
So, Eui Young; Ouchi, Toru (2013) The Potential Role of BRCA1-Associated ATM Activator-1 (BRAT1) in Regulation of mTOR. J Cancer Biol Res 1:
So, Eui Young; Ouchi, Toru (2010) The application of Toll like receptors for cancer therapy. Int J Biol Sci 6:675-81
Shukla, Vivek; Coumoul, Xavier; Lahusen, Tyler et al. (2010) BRCA1 affects global DNA methylation through regulation of DNMT1. Cell Res 20:1201-15
Saeki, Toshiaki; Ouchi, Mutsuko; Ouchi, Toru (2009) Physiological and oncogenic Aurora-A pathway. Int J Biol Sci 5:758-62