Abstract

Regulation of normal cell proliferation in higher eucaryotes is strongly linked to expression of the c-myc proto-oncogene. Abnormal expression of the c-myc gene, in certain cases, appear to be associated with the process of tumorigenesis. Therefore, understanding how transcription of the c-myc gene is regulated will lead to a better understanding of the mechanisms controlling both normal and abnormal cell proliferation. Transcription of the murine c-myc gene is regulated in part by sequences that flank the major promoter (P2). These include enhancer and dehancer/repressor-like elements located at a distance from the c-myc transcription start site. Upstream promoter elements that are close to the start sit play an essential role in regulating transcription in most promoters. However, a detailed analysis of these upstream promoter elements in the P2 promoter of the c-myc gene has not been forthcoming. Here, an in vitro transcription system was used as a starting point in an analysis of the upstream promoter elements in the P2 promoter of the murine c-myc gene. It was found that sequences between -113 to -24 relative to P2 contain the information necessary for maximal transcription in vitro. Within this region are multiple protein binding sites i.e. ME1a, UBP and putative SP1). Optimal transcription in vitro appears to be dependent on the binding of at least some of these factors. The ME1a element alone can increase transcription initiation from P2 and appears to be a novel promoter element. Further, the binding of a protein(s) to the ME1a element is significantly increased in extracts from serum stimulated fribroblasts. This grant proposes to continue this analysis of the upstream promoter elements in the P2 promoter of the murine c-myc gene. The long term goal is to define and characterize the elements and factors that are essential for transcription in the specific region 113 bases 5' of P2. Towards this end two broad objectives are proposed. The first objective is to further define the cis-acting elements adjacent to P2 that are necessary for transcription in vitro and in vivo. The goal is to determine how transcription is dependent on the position, orientation and arrangement of the UBP, SP1 and ME1a elements. The second objective is to isolate, purify and characterize the ME1a binding protein, isolate its cognate cDNA and determine whether this protein acts as a transcription factor.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
First Independent Research Support & Transition (FIRST) Awards (R29)
Project #
5R29CA051170-04
Application #
3459734
Study Section
Molecular Biology Study Section (MBY)
Project Start
1989-12-01
Project End
1994-11-30
Budget Start
1992-12-01
Budget End
1993-11-30
Support Year
4
Fiscal Year
1993
Total Cost
Indirect Cost

  Institution

Name
Thomas Jefferson University
Department
Type
Schools of Medicine
DUNS #
061197161
City
Philadelphia
State
PA
Country
United States
Zip Code
19107

  Publications

Stubbs, M C; Min, I; Izzo, M W et al. (2000) The ZF87/MAZ transcription factor functions as a growth suppressor in fibroblasts. Biochem Cell Biol 78:477-85
Min, I; Stubbs, M C; Strachan, G D et al. (1998) Cyclin A levels, the duration of S phase and sensitivity to a chemotherapeutic agent are altered in fibroblasts cultured on a fibronectin matrix. Int J Oncol 13:549-55
Jordan-Sciutto, K L; Hall, D J (1998) A mutant E2F-1 transcription factor that affects the phenotype of NIH3T3 fibroblasts inefficiency associates with cyclin A-cdk2. Biochem Cell Biol 76:37-44
Logan, T J; Jordan, K L; Evans, D L et al. (1997) Altered cell shape is linked to increased p34cdc2 gene expression in fibroblasts expressing a mutant E2F-1 transcription factor. J Cell Biochem 65:83-94
Logan, T J; Moberg, K H; Hall, D J (1997) Multiprotein complex formation on the c-myc promoter. Biochem Mol Biol Int 43:945-53
Jordan-Sciutto, K L; Logan, T J; Norton, P A et al. (1997) Reduction in fibronectin expression and alteration in cell morphology are coincident in NIH3T3 cells expressing a mutant E2F1 transcription factor. Exp Cell Res 236:527-36
Jordan, K L; Evans, D L; Steelman, S et al. (1996) Isolation of two novel cDNAs whose products associate with the amino terminus of the E2F1 transcription factor. Biochemistry 35:12320-8
Logan, T J; Jordan, K L; Hall, D J (1996) Constitutive expression of the E2F1 transcription factor in fibroblasts alters G0 and S phase transit following serum stimulation. Biochem Cell Biol 74:21-8
Logan, T J; Evans, D L; Mercer, W E et al. (1995) Expression of a deletion mutant of the E2F1 transcription factor in fibroblasts lengthens S phase and increases sensitivity to S phase-specific toxins. Cancer Res 55:2883-91
Jordan, K L; Haas, A R; Logan, T J et al. (1994) Detailed analysis of the basic domain of the E2F1 transcription factor indicates that it is unique among bHLH proteins. Oncogene 9:1177-85

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