Abstract

The transforming growth factor 2 (TGF2) signaling controls many cellular processes including cell proliferation and apoptosis and is critical for maintaining tissue homeostasis. Aberrant levels of TGF2 signaling lead to defective tissue regeneration and various human diseases such as cancer. The long-term goal of this project is to understand how proper levels of TGF2 signaling activity are maintained and regulated in normal tissues and primary cells using a system biology approach. The goal of this application is to develop a comprehensive mathematical model that can be used to predict Smad signaling dynamics and behavior and to determine the function of SnoN-mediated negative feedback regulation of Smad signaling. We will employ primary hepatocytes from wild type and SnoN-null mice to perform quantitative measurement and establish a mathematical model, and further confirm the model in liver tissue sections. We choose to work with liver because TGF2 is known to be a potent inhibitor of hepatocyte proliferation and is also the critical negative regulator of liver regeneration. In primary hepatocytes, TGF2 signals through Smad2 and Smad4 proteins. Upon phosphorylation by the active TGFss receptor kinases, Smad2 homo-oligomerizes and heterooligomerizes with Smad4, leading to its accumulation in the nucleus. The heteromeric Smad2/Smad4 complex then interacts with other transcription factors to regulate expression of TGF2-responsive genes. The activities of the Smad proteins are regulated by positive and negative cellular co-factors. Through a system biology study, we have recently determined that SnoN is the most important negative regulator of Smad signaling in primary hepatocytes. SnoN binds to Smad2 and Smad4 and represses their ability to activate TGF2 target genes. Interestingly, SnoN itself is induced by TGF2, suggesting that it modulates TGF2 signaling in a negative feedback manner. Our preliminary study suggests that SnoN neither affects the duration nor the initial timing of Smad signaling, but rather decreases the level of target gene expression at high TGF2 concentrations. We hypothesize that the SnoN-mediated negative feedback functions to suppress cell-to-cell variability in Smad target gene expression and linearize dose-response behavior of TGF2 signaling, thereby maintaining the robustness of this signaling pathway. In this proposal we will combine mathematical modeling with quantitative measurements to test this hypothesis at both the cellular level, using primary hepatocytes, and at the organ level, using liver tissues from wild type and snoN mutant mice.
Three specific aims have been proposed: 1) Analysis of the impact of SnoN on TGF2 signaling in primary hepatocytes. 2) Analysis of the effects of SnoN on Smad-dependent gene expression. 3) Modeling SnoN regulation of Smad signaling during liver damage and regeneration. This study will significantly advance our knowledge regarding the mechanism and regulation of this important signaling pathway and how de-regulation of this signaling activity results in carcinogenesis.

Public Health Relevance

The transforming growth factor 2 (TGF2) signaling controls many cellular processes and is critical for maintaining tissue homeostasis. Aberrant levels of TGF2 signaling lead to defective tissue regeneration and various human diseases such as cancer and diabetes. The long-term goal of this project is to understand how proper levels of TGF2 signaling activity are maintained and regulated in normal tissues and primary cells using a system biology approach.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
1R01DK090347-01
Application #
8026358
Study Section
Modeling and Analysis of Biological Systems Study Section (MABS)
Program Officer
Serrano, Jose
Project Start
2011-01-05
Project End
2014-12-31
Budget Start
2011-01-05
Budget End
2011-12-31
Support Year
1
Fiscal Year
2011
Total Cost
$339,430
Indirect Cost

  Institution

Name
University of California Berkeley
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
124726725
City
Berkeley
State
CA
Country
United States
Zip Code
94704

  Publications

Strasen, Jette; Sarma, Uddipan; Jentsch, Marcel et al. (2018) Cell-specific responses to the cytokine TGF? are determined by variability in protein levels. Mol Syst Biol 14:e7733
Rashidian, Juliet; Luo, Kunxin (2016) Three-dimensional Mammary Epithelial Cell Morphogenesis Model for Analysis of TGFß Signaling. Methods Mol Biol 1344:121-35
Marwitz, Sebastian; Depner, Sofia; Dvornikov, Dmytro et al. (2016) Downregulation of the TGF? Pseudoreceptor BAMBI in Non-Small Cell Lung Cancer Enhances TGF? Signaling and Invasion. Cancer Res 76:3785-801
Rashidian, Juliet; Le Scolan, Erwan; Ji, Xiaodan et al. (2015) Ski regulates Hippo and TAZ signaling to suppress breast cancer progression. Sci Signal 8:ra14
Ji, Xiaodan; Lu, Huasong; Zhou, Qiang et al. (2014) LARP7 suppresses P-TEFb activity to inhibit breast cancer progression and metastasis. Elife 3:e02907
Zhu, Qingwei; Kim, Yong Hwan; Wang, Douglas et al. (2013) SnoN facilitates ALK1-Smad1/5 signaling during embryonic angiogenesis. J Cell Biol 202:937-50
Jahchan, Nadine S; Ouyang, Gaoliang; Luo, Kunxin (2013) Expression profiles of SnoN in normal and cancerous human tissues support its tumor suppressor role in human cancer. PLoS One 8:e55794
Pan, Deng; Zhu, Qingwei; Conboy, Michael J et al. (2012) SnoN activates p53 directly to regulate aging and tumorigenesis. Aging Cell 11:902-911
Zhu, Qingwei; Luo, Kunxin (2012) SnoN in regulation of embryonic development and tissue morphogenesis. FEBS Lett 586:1971-6
Deheuninck, Julien; Luo, Kunxin (2009) Ski and SnoN, potent negative regulators of TGF-beta signaling. Cell Res 19:47-57