A novel factor distinct from E2F mediates C-MYC promoter activation through its E2F element during exit from quiescence

doi:10.1093/carcin/bgp002

Carcinogenesis Advance Access published online on January 6, 2009
Carcinogenesis, doi:10.1093/carcin/bgp002

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A novel factor distinct from E2F mediates C-MYC promoter activation through its E2F element during exit from quiescence

Josué Álvaro-Blanco¹, Lorena Martínez-Gac¹, Esther Calonge², María Rodríguez-Martínez¹, Irene Molina-Privado¹, Juan M. Redondo³, José Alcamí², Erik K. Flemington⁴ and Miguel R. Campanero¹^,*

¹ Instituto de Investigaciones Biomédicas, Consejo Superior de Investigaciones Científicas y Universidad Autónoma de Madrid; Arturo Duperier, 4; 28029 Madrid, Spain
² Unidad de Inmunopatología del Sida; Centro Nacional de Microbiología; Instituto de Salud Carlos III; Carretera de Majadahonda a Pozuelo; Majadahonda; 28220 Madrid, Spain
³ Centro Nacional de Investigaciones Cardiovasculares; Melchor Fernandez Almagro, 3; 28029 Madrid, Spain
⁴ Tulane Health Sciences Center; 1430 Tulane Ave.; New Orleans, LA 70112; USA

^* To whom correspondence should be addressed: Address correspondence to: Tel: 34-91-585-4490; Fax: 34-91-585-4401; Email: mcampanero{at}iib.uam.es

Although C-MYC is over-expressed in a number of tumors, themechanisms governing its expression in normal or tumor cellsare not completely understood. Recruitment of the Retinoblastomaprotein family members to gene promoters by E2F factors hasa dominant negative effect on their activity during the G0 andG1 phases of the cell cycle. Despite the presence of an E2Fbinding-site on the C-MYC promoter, it escapes the repressiveeffect of E2F-Retinoblastoma complexes through unknown mechanismsduring exit from quiescence. We hypothesized that occupancyof E2F elements by factors distinct from E2F might account forthis escape. To test this hypothesis, we investigated whetherthe E2F element in the C-MYC promoter is regulated differentlythan E2F elements in promoters that are activated at the G₁-Stransition. Employing gel shift analysis, the E2F element fromthe C-MYC promoter was found to form a unique non-E2F complex,referred to as EMYCS, which is not observed with E2F elementsfrom several other promoters. The DNA contact residues for EMYCSare distinct but overlapping with residues required for bindingof E2F proteins. Finally, the approximate estimated molecularweight of the DNA binding component of EMCYS is 105 kDa. Functionalstudies indicate that EMYCS has transcriptional transactivationcapacity and suggest that it is required to activate the C-MYCpromoter during exit from quiescence.

Received July 4, 2008; revised December 11, 2008; accepted December 26, 2008.

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