Induction of the Cellular E2F-1 Promoter by the Adenovirus E4-6/7 Protein
Autor: | Patrick Hearing, Laura J. Taylor, Dafna Bar-Sagi, Robert J. O'Connor, Joel E Schaley |
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Jazyk: | angličtina |
Rok vydání: | 2000 |
Předmět: |
Gene Expression Regulation
Viral Immunology Molecular Sequence Data Repressor Cell Cycle Proteins Biology Microbiology Adenoviridae Cell Line Retinoblastoma-like protein 1 Transactivation Virology Humans Amino Acid Sequence Binding site Cloning Molecular E2F Promoter Regions Genetic Transcription factor Electrophoresis Agar Gel Reporter gene Binding Sites Promoter DNA Molecular biology Immunohistochemistry Recombinant Proteins Virus-Cell Interactions E2F Transcription Factors DNA-Binding Proteins stomatognathic diseases Insect Science biological phenomena cell phenomena and immunity Carrier Proteins Sequence Alignment Transcription Factor DP1 E2F1 Transcription Factor Adenovirus E4 Proteins HeLa Cells Retinoblastoma-Binding Protein 1 Transcription Factors |
Popis: | The adenovirus type 5 (Ad5) E4-6/7 protein interacts directly with different members of the E2F family and mediates the cooperative and stable binding of E2F to a unique pair of binding sites in the Ad5 E2a promoter region. This induction of E2F DNA binding activity strongly correlates with increased E2a transcription when analyzed using virus infection and transient expression assays. Here we show that while different adenovirus isolates express an E4-6/7 protein that is capable of induction of E2F dimerization and stable DNA binding to the Ad5 E2a promoter region, not all of these viruses carry the inverted E2F binding site targets in their E2a promoter regions. The Ad12 and Ad40 E2a promoter regions bind E2F via a single binding site. However, these promoters bind adenovirus-induced (dimerized) E2F very weakly. The Ad3 E2a promoter region binds E2F very poorly, even via a single binding site. A possible explanation of these results is that the Ad E4-6/7 protein evolved to induce cellular gene expression. Consistent with this notion, we show that infection with different adenovirus isolates induces the binding of E2F to an inverted configuration of binding sites present in the cellular E2F-1 promoter. Transient expression of the E4-6/7 protein alone in uninfected cells is sufficient to induce transactivation of the E2F-1 promoter linked to chloramphenicol acetyltransferase or green fluorescent protein reporter genes. Further, expression of the E4-6/7 protein in the context of adenovirus infection induces E2F-1 protein accumulation. Thus, the induction of E2F binding to the E2F-1 promoter by the E4-6/7 protein observed in vitro correlates with transactivation of E2F-1 promoter activity in vivo. These results suggest that adenovirus has evolved two distinct mechanisms to induce the expression of the E2F-1 gene. The E1A proteins displace repressors of E2F activity (the Rb family members) and thus relieve E2F-1 promoter repression; the E4-6/7 protein complements this function by stably recruiting active E2F to the E2F-1 promoter to transactivate expression. |
Databáze: | OpenAIRE |
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