ulate the expression of numerous genes, the best known being the Hox genes. Drosophila Hox genes contain PREs/TREs that serve as platforms for the recruitment of the PcG/trxG protein complexes. Binding of PcG/trxG proteins at these sites leads to transcriptional regulation via post-translational modification of histones. These modifications can have antagonistic effects on transcription. For example, the monoubiquitylation of histone H2A mediated by the E3-ubiquitin ligase SCE/dRING promotes transcriptional repression while the monoubiquitylation of histone H2B mediated by the E3-ubiquitin ligase dBRE1 promotes transcriptional activation. The dBRE1 protein forms a complex with RAD6 which is required to promote H2B ubiquitylation, a prerequisite for the H3K4 methylation that promotes transcriptional activation. SCE/dRING is a core subunit of the repressor PRC1 complex that also contains Polycomb, Posterior Sex Comb and Polyhomeotic. Knowledge of the compositional diversity of PRC1 is expanding and variants of PRC1 and non-canonical PRC1 complexes with distinct transcriptional outcomes have been isolated. For example, the dRAF complex composed of dRING, PSC and dKDM2 promotes stronger repression than PRC1 as it stimulates monoubiquitylation of H2A more efficiently and also demethylates H3K36me2, a modification established by trxG. Moreover, recent results in vertebrates indicate the existence of non-canonical PRC1 complexes that, instead of containing the core subunit PC they contain the RYBP subunit forming the PRC1-RYBP complexes found to locate at target genes with intermediate levels of expression. The finding of non-canonical PRC1 complexes has led to recent discoveries that are challenging the classical hierarchical recruitment complex model whereby PRC1 complex is recruited by PRC2-mediated H3K27 trimethylation. It has now been shown in vertebrates that non-canonical PRC1-mediated H2A monoubiquitylation can recruit PRC2. The conserved dRYBP/YAF2/RYBP protein contains in its N-terminal a Ubiquitin Binding Domain of the type Nucleoporin Zinc Finger and the murine RYBP has been shown to interact with ubiquitin. Loss of dRYBP function in Drosophila produces a range of phenotypes that are highly variable in penetrance suggesting that dRYBP functions in a range of biological processes. Moreover, although dRYBP inactivation does not produce homeotic phenotypes, dRYBP has been shown to interact with PcG/trxG proteins and to function as a PcG-dependent transcriptional repressor. However, the mechanisms INK1117 chemical information underlying dRYBP function in epigenetic regulation of gene expression mediated by PcG/trxG proteins remain poorly PubMed ID:http://www.ncbi.nlm.nih.gov/pubmed/19692147 understood. 2 / 17 dRYBP Counteracts Activation and Repression Here we show that dRYBP interacts genetically PubMed ID:http://www.ncbi.nlm.nih.gov/pubmed/19691363 and biochemically with dRING, dKDM2 and dBRE1 to modulate H2Aub, H3K36me2 and H2Bub levels and thereby regulate gene repression and activation. Results and Discussion dRYBP interacts with ubiquitin and with ubiquitylated proteins The dRYBP protein sequence suggests its function in the process of ubiquitylation, a crucial step in the epigenetic regulation of transcription. We first analyzed whether dRYBP binds ubiquitin. We performed immunoprecipitation of Drosophila wild type nuclear protein extracts using antidRYBP antibody and the samples were analyzed by immunoblotting with antiubiquitin and anti-dRYBP antibodies. 3 / 17 dRYBP Counteracts Activation and Repression The dRYBP protein associates with SCE, dKDM2 and dBRE1 We
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