In silico identification of transcriptional regulators associated with c-Myc

doi:10.1093/nar/gkh816

Nucleic Acids Research 2004 32(17):4955-4961; doi:10.1093/nar/gkh816

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Published online 23 September 2004

In silico identification of transcriptional regulators associated with c-Myc

Ran Elkon, Karen I. Zeller², Chaim Linhart¹, Chi V. Dang²^,3, Ron Shamir¹ and Yosef Shiloh^*

The David and Inez Myers Laboratory for Genetic Research, Department of Human Genetics, Sackler School of Medicine, ¹ School of Computer Science, Tel Aviv University, Israel, ² Division of Hematology, Department of Medicine and ³ The Sidney Kimmel Comprehensive Cancer Center, Johns Hopkins University School of Medicine, Baltimore, MD 21212 USA

^* To whom correspondence should be addressed at Department of Human Genetics and Molecular Medicine, Sackler School of Medicine, Room 1002, Tel Aviv University, Ramat Aviv 69978, Israel. Tel: +972 3 6409760; Fax: +972 3 6407471; Email: yossih{at}post.tau.ac.il

Received July 22, 2004; Revised and Accepted August 21, 2004

The development of powerful experimental strategies for functionalgenomics and accompanying computational tools has brought majoradvances in the delineation of transcriptional networks in organismsranging from yeast to human. Regulation of transcription ofeukaryotic genes is to a large extent combinatorial. Here, weused an in silico approach to identify transcription factors(TFs) that form recurring regulatory modules with c-Myc, a proteinencoded by an oncogene that is frequently disregulated in humanmalignancies. A recent study identified, on a genomic scale,human genes whose promoters are bound by c-Myc and its heterodimerpartner Max in Burkitt's lymphoma cells. Using computationalmethods, we identified nine TFs whose binding-site signaturesare highly overrepresented in this promoter set of c-Myc targets,pointing to possible functional links between these TFs andc-Myc. Binding sites of most of these TFs are also enrichedon the set of mouse homolog promoters, suggesting functionalconservation. Among the enriched TFs, there are several regulatorsknown to control cell cycle progression. Another TF in thisset, EGR-1, is rapidly activated by numerous stress challengesand plays a central role in angiogenesis. Experimental investigationconfirmed that c-Myc and EGR-1 bind together on several targetpromoters. The approach applied here is general and demonstrateshow computational analysis of functional genomics experimentscan identify novel modules in complex networks of transcriptionalregulation.

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