Abstract

The liver is one of the few adult organs capable of completely regenerating itself in response to cellular injury from toxins, viral infections or tissue removal. The long term goal of this proposal is to understand the role of proliferation- and hepatocyte-specific transcription factors mediating replication during liver regeneration. Transcriptional regulation of hepatocyte-specific gene expression relies on combinatorial interaction of multiple DNA binding sites by several distinct hepatocyte nucleus factors (HNF). Regeneration of the liver following injury involves a balance between hepatocyte proliferation plus sustained expression of hepatocyte-specific genes required for homeostasis and simultaneously diminishing the transcription of cell- specific genes that may interfere with hepatocyte replication. Although the mechanisms involved in this transcriptional decline remain uncharacterized, the cut-homeodomain HNF-6 protein is likely to be involved because it is one of the few hepatocyte-specific transcription factors whose expression is reduced during liver regeneration. Furthermore, a number of potential HNF-6 target genes decline during liver regeneration, several of which may inhibit hepatocyte replication. A transgenic mouse line will be generated in which decreased HFN-6 expression during liver regeneration can be prevented. We will use these mice to test the hypothesis that undiminished HFN-6 expression is inhibitory to liver regeneration. The immediate early gene expression that is induced during liver regeneration is known to mediate hepatocyte progression into the G1 stage of the cell-cycle. However, the transcriptional mechanisms mediating the later stages of hepatocyte replication are not completely understood. To further examine transcriptional processes underlying cell cycle progression during liver regeneration, we will alter hepatocyte expression of the winged helix HNF-3/fork head homolog-11 (HFH-11) gene. HFH-11 is a candidate transcription factor involved in cell cycle progression because its expression is transiently reactivated during the period of hepatocyte proliferation, and putative HFH-11 binding sites are present in cell- cycle regulatory genes such as c-myc, c-myb, TGFalpha, cyclin B1 and cyclin D1. We will generate mice possessing a conditional targeted HFH- 11 gene disruption in adult hepatocytes and liver regeneration studies with these mice will allow us to test the hypothesis that HFH-11 expression is necessary for hepatocyte replication. Gain of function studies in transgenic mice are proposed to examine whether premature hepatocyte expression of HFH-11 during liver regeneration results in altered cell cycle kinetics of proliferating hepatocytes. Assessment of these transgenic mice for development of liver nodules in a liver tumor promotion model will allow us to investigate whether continuous hepatocyte expression of HFH-11 increases the incidence of hepatocellular carcinoma. An understanding of transcriptional mechanisms which mediate liver regeneration may allow us to identify regulatory pathways that are potentially disrupted during liver fibrosis and cirrhosis.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK054687-02
Application #
6164534
Study Section
Metabolic Pathology Study Section (MEP)
Program Officer
Serrano, Jose
Project Start
1999-03-15
Project End
2004-02-29
Budget Start
2000-03-01
Budget End
2001-02-28
Support Year
2
Fiscal Year
2000
Total Cost
$315,764
Indirect Cost

  Institution

Name
University of Illinois at Chicago
Department
Biochemistry
Type
Schools of Medicine
DUNS #
121911077
City
Chicago
State
IL
Country
United States
Zip Code
60612

  Publications

Petrovic, Vladimir; Costa, Robert H; Lau, Lester F et al. (2010) Negative regulation of the oncogenic transcription factor FoxM1 by thiazolidinediones and mithramycin. Cancer Biol Ther 9:1008-16
Chen, Yi-Ju; Dominguez-Brauer, Carmen; Wang, Zebin et al. (2009) A conserved phosphorylation site within the forkhead domain of FoxM1B is required for its activation by cyclin-CDK1. J Biol Chem 284:30695-707
Wang, I-Ching; Chen, Yi-Ju; Hughes, Douglas E et al. (2008) FoxM1 regulates transcription of JNK1 to promote the G1/S transition and tumor cell invasiveness. J Biol Chem 283:20770-8
Petrovic, Vladimir; Costa, Robert H; Lau, Lester F et al. (2008) FoxM1 regulates growth factor-induced expression of kinase-interacting stathmin (KIS) to promote cell cycle progression. J Biol Chem 283:453-60
Wang, I-C; Meliton, L; Tretiakova, M et al. (2008) Transgenic expression of the forkhead box M1 transcription factor induces formation of lung tumors. Oncogene 27:4137-49
Park, Hyun Jung; Costa, Robert H; Lau, Lester F et al. (2008) Anaphase-promoting complex/cyclosome-CDH1-mediated proteolysis of the forkhead box M1 transcription factor is critical for regulated entry into S phase. Mol Cell Biol 28:5162-71
Park, H J; Wang, Z; Costa, R H et al. (2008) An N-terminal inhibitory domain modulates activity of FoxM1 during cell cycle. Oncogene 27:1696-704
Brezillon, Nicolas; Lambert-Blot, Martine; Morosan, Serban et al. (2007) Transplanted hepatocytes over-expressing FoxM1B efficiently repopulate chronically injured mouse liver independent of donor age. Mol Ther 15:1710-5
Gusarova, Galina A; Wang, I-Ching; Major, Michael L et al. (2007) A cell-penetrating ARF peptide inhibitor of FoxM1 in mouse hepatocellular carcinoma treatment. J Clin Invest 117:99-111
Kotlo, Kumar; Hughes, Douglas E; Herrera, Victoria L M et al. (2007) Functional polymorphism of the Anpep gene increases promoter activity in the Dahl salt-resistant rat. Hypertension 49:467-72

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