Abstract

The long term objectives of this proposal is to understand the establishment and maintenance of liver-specific gene transcription during development. Evidence is accumulating that the establishment of the differential transcription of tissue-specific genes during development from the same genomic DNA is regulated by a cascade of transcription factors. Therefore, the establishment of tissue specific gene expression involves the execution of a network of temporally controlled transcription factors whose function are necessary to program the transcription of different genes in each cell-type in the body. The DNA regulatory regions of tissue- specific genes consist of multiple DNA elements that stimulate expression through the interaction with cell-specific transcription factors. This reinforces the importance of deciphering the mechanisms that restrict activity of cell-specific transcription factors and of the analyses of functional protein domains involved in transcriptional activation. To initiate experiments toward these goals, the characterization of two liver- specific transcription factors (termed hepatocyte nuclear factors; HNF) that regulate the expression of the transthyretin (TTR) gene will be performed. The two transcription factors, HNF 3 and HNF 4, that will be analyzed in this proposal also participate in coordinate expression of several other unrelated genes in the liver. Therefore they are involved in the general regulation of liver genes. they availability of the HNF 3 cDNA clone will allow initiation of these studies and the isolation of the clone encoding HNF 4 will expand this analysis. The expression of these HNF cDNA will allow the synthesis of specific antisera that is critical for the identification of protein-protein interactions and the investigation of the cellular distribution of these factors. The HNF cDNAs and antibodies will be used to determine whether transcriptional or translational mechanisms maintain the activity of these factors restricted to hepatocytes. The mechanism which limits their activity is important for the understanding of hepatocyte-specific expression, since this property prevents the expression of these liver genes in other cell-types. Future extension of these studies will involve the investigation of the cascade schemes that regulate the HNF cell-specific activity. The HNF clones are also used to construct deletion mutations to identify functional protein domains involved in DNA recognition and possible protein-protein interactions. In addition these HNF deletion mutations are used in a cotransfection assay with a test gene that requires HNF activity for expression to delineate protein domains involved in transcriptional activation. Since deletion within the HNF coding region may disrupt protein structure, the functional domains are confirmed by site-directed mutations which alter only several amine acid residues. These mutations will also provide insight into the type of amino acid sequence that is required for the functional activity. These studies will strengthen our understanding of the molecular basis controlling tissue-specific gene transcription.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM043241-03
Application #
3302256
Study Section
Physiological Chemistry Study Section (PC)
Project Start
1990-07-01
Project End
1995-06-30
Budget Start
1992-07-01
Budget End
1993-06-30
Support Year
3
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

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

  Publications

Tan, Yongjun; Yoshida, Yuichi; Hughes, Douglas E et al. (2006) Increased expression of hepatocyte nuclear factor 6 stimulates hepatocyte proliferation during mouse liver regeneration. Gastroenterology 130:1283-300
Yoshida, Yuichi; Hughes, Douglas E; Rausa 3rd, Francisco M et al. (2006) C/EBPalpha and HNF6 protein complex formation stimulates HNF6-dependent transcription by CBP coactivator recruitment in HepG2 cells. Hepatology 43:276-86
Costa, Robert H; Kalinichenko, Vladimir V; Major, Michael L et al. (2005) New and unexpected: forkhead meets ARF. Curr Opin Genet Dev 15:42-8
Wang, Minhua; Tan, Yongjun; Costa, Robert H et al. (2004) In vivo regulation of murine CYP7A1 by HNF-6: a novel mechanism for diminished CYP7A1 expression in biliary obstruction. Hepatology 40:600-8
Rausa 3rd, Francisco M; Hughes, Douglas E; Costa, Robert H (2004) Stability of the hepatocyte nuclear factor 6 transcription factor requires acetylation by the CREB-binding protein coactivator. J Biol Chem 279:43070-6
Sheng, Wanyun; Yan, Hong; Rausa 3rd, Francisco M et al. (2004) Structure of the hepatocyte nuclear factor 6alpha and its interaction with DNA. J Biol Chem 279:33928-36
Rausa, Francisco M; Tan, Yongjun; Costa, Robert H (2003) Association between hepatocyte nuclear factor 6 (HNF-6) and FoxA2 DNA binding domains stimulates FoxA2 transcriptional activity but inhibits HNF-6 DNA binding. Mol Cell Biol 23:437-49
Costa, Robert H; Kalinichenko, Vladimir V; Holterman, Ai-Xuan L et al. (2003) Transcription factors in liver development, differentiation, and regeneration. Hepatology 38:1331-47
Hughes, Douglas E; Stolz, Donna Beer; Yu, Songtao et al. (2003) Elevated hepatocyte levels of the Forkhead box A2 (HNF-3beta) transcription factor cause postnatal steatosis and mitochondrial damage. Hepatology 37:1414-24
Guo, Ying; Costa, Robert; Ramsey, Heather et al. (2002) The embryonic stem cell transcription factors Oct-4 and FoxD3 interact to regulate endodermal-specific promoter expression. Proc Natl Acad Sci U S A 99:3663-7

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