ad cellular functions fol lowing activation of MYC. The majority of MYC responsive genes were involved in metabolic, transcrip tional, transportational and signal transduction pathways. Genes involved in post transcrip tional modification and post translational modification were also thoroughly significantly enriched. Similarly, a significant enrichment of genes relating to ribosome biogenesis was detected, suggestive of MYCs recently elucidated role as a regulator of ribo some biogenesis and protein synthesis. As expected given the role of MYC in proliferation, genes involved in cell cycle progression were amongst the most signifi cantly enriched. Genes involved in apoptosis and DNA damage checkpoint pathways were Inhibitors,Modulators,Libraries also enriched, along with genes involved in related functions such as cellular response to stress and cytoskeleton organisation.
Enrichment of GO terms Inhibitors,Modulators,Libraries for MYC responsive genes showing early changes in expression for the pan creas and skin identified similar numbers for both tissues, with the exception of genes relating to DNA damage and DNA replication, where a larger number of genes are detected for the pancreas than for the skin. These results indicate that whilst expression of genes relating to multiple cellular functions is common to both tissues, expression of genes involved in DNA damage and repli cation is more specific to the b cells. Expression of putative MYC target genes following MYC ERTAM Inhibitors,Modulators,Libraries activation The MYC Target Gene Database currently identi fies 1,697 genes as putative MYC targets. Inhibitors,Modulators,Libraries Of these, 13. 4% and 19.
2% were found to be both MYC respon Drug_discovery sive and show a 2 fold change in expression in the skin and pancreas respectively within 8 hours. The predominant role for these genes was in DNA replication, biosynthesis, metabolism, cell cycle, cell division and other related functions. Cellular func tions relating to apoptosis and cell death were also highly enriched, although to a lesser degree than those relating to cellular proliferation. These data suggest that activation of the MYC ERTAM protein in vivo leads to a rapid change in the expression of a large number of putative MYC targets. However, known target genes represent only a small fraction of detected MYC respon sive genes, indicating that the majority of these observed expression changes may be downstream of direct MYC induced transcription.
To identify the level of overlap between the genes classed as significantly altered in this study and those www.selleckchem.com/products/BAY-73-4506.html identified in previous analyses, we utilised the Gene Set Enrichment Analysis program developed by the Broad Institute. This allowed us to identify gene sets in which significant differentially expressed genes are enriched. Gene sets were taken from the Molecular Signatures Database, as well as from addi tional published datasets. Additional file 1, Table S7 and Additional file 1, Table S8 show the results from GSEA for the genes showing significant expres sion at the early time points for the pancreas and skin, respectively. These