Abstract

Our long-term goal is to understand in detail the molecular mechanisms involved in cell transformation by the human adenoviruses. To accomplish this objective, We propose to identify and analyze cellular genes that regulate the transformed phenotype and to study mechanisms of interaction between the Ad T antigens and cellular and viral macromolecules.
Our specific aims are the following: 1. To identify cellular genes that may be positively or negatively regulated in Ad-transformed cells. We will construct and analyze extensive random and hybridization-subtracted cDNA libraries in AGT10 from parallel Ad-transformed and parental non-transformed cells and screen cDNA libraries with a sensitivity to detect expression of single-copy genes (1 mRNA in 100,000). 2. To prove that the modified expression of specific cellular genes is a function of E1A or E1B T antigen synthesis. We will generate and analyze stable cell lines containing individual Ad E1A and E1B genes regulated by inducible promoters. 3. To study structure and function of highly purified, in vitro phosphorylated, E. coli-produced Ad12 E1A 266R (13S mRNA) and 235R (12S mRNA) T antigens. We will determine whether phosphorylated T antigen binds to specific DNA sequences and regulates transcription in vitro. 4. To identify and isolate putative cellular (and viral) proteins and nucleic acids that associate with E1A T antigens within cells and that bind to purified phosphorylated Ad12 E1A antigens in vitro. 5. To determine the domains of the E1A T antigens that are responsible for the immortalization and partial transformation functions. We will study Ad E1A single base-pair mutants that saturate specific domains of E1A T antigens. 6. To identify and study known and theoretical adenovirus proteins. We will synthesize antipeptide antibodies targeted to putative URF 10 and URF 11 proteins encoded in Ad2 E1 1-strand, putative 6.1K protein encoded by the Ad2 E1A-9S mRNA, early Ad2 L1 52K/55K protein(s), putative Ad2 angnoprotein encoded at 21-22.5 mu and putative Ad2 protease at 60.0-61.7. We will use antipeptide antibodies to analyze the corresponding viral proteins and to study mutants in URF 10, URF 11, and L1 52K/55K.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA029561-32
Application #
3168762
Study Section
Virology Study Section (VR)
Project Start
1980-08-01
Project End
1991-05-31
Budget Start
1989-06-01
Budget End
1991-05-31
Support Year
32
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
Saint Louis University
Department
Type
Schools of Medicine
DUNS #
City
Saint Louis
State
MO
Country
United States
Zip Code
63103

  Publications

Loewenstein, Paul M; Wu, Shwu-Yuan; Chiang, Cheng-Ming et al. (2012) The adenovirus E1A N-terminal repression domain represses transcription from a chromatin template in vitro. Virology 428:70-5
Loewenstein, Paul M; Green, Maurice (2011) Expression of the Adenovirus Early Gene 1A Transcription-Repression Domain Alone Downregulates HER2 and Results in the Death of Human Breast Cancer Cells Upregulated for the HER2 Proto-Oncogene. Genes Cancer 2:737-44
Green, Maurice; Panesar, Ninder K; Loewenstein, Paul M (2008) Adenovirus E1A proteins are closely associated with chromatin in productively infected and transformed cells. Virology 371:1-7
Green, M; Panesar, N K; Loewenstein, P M (2008) The transcription-repression domain of the adenovirus E1A oncoprotein targets p300 at the promoter. Oncogene 27:4446-55
Green, Maurice; Thorburn, Andrew; Kern, Robert et al. (2007) The use of cell microinjection for the in vivo analysis of viral transcriptional regulatory protein domains. Methods Mol Med 131:157-86
Loewenstein, Paul M; Song, Chao-Zhong; Green, Maurice (2007) The use of in vitro transcription to probe regulatory functions of viral protein domains. Methods Mol Med 131:15-31
Loewenstein, Paul M; Arackal, Sophia; Green, Maurice (2006) Mutational and functional analysis of an essential subdomain of the adenovirus E1A N-terminal transcription repression domain. Virology 351:312-21
Boyd, Janice M; Loewenstein, Paul M; Tang Qq, Qing-quan et al. (2002) Adenovirus E1A N-terminal amino acid sequence requirements for repression of transcription in vitro and in vivo correlate with those required for E1A interference with TBP-TATA complex formation. J Virol 76:1461-74
Song, C Z; Loewenstein, P M; Toth, K et al. (1997) The adenovirus E1A repression domain disrupts the interaction between the TATA binding protein and the TATA box in a manner reversible by TFIIB. Mol Cell Biol 17:2186-93
Song, C Z (1996) Requirement for phosphorylation of RNA polymerase II C-terminal domain in transcription is both transcript length and promoter dependent. Biochem Biophys Res Commun 229:810-6

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