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Fmoc-Ala-OH mg To validate the effects of the G a
To validate the effects of the G9a HMT inhibitors on HMEC-1 Fmoc-Ala-OH mg and transcriptional responses we generated knockdown cells for G9a using an shRNA approach. Upon transduction of HMEC-1 and doxycycline activation of the shRNA, both G9a HMT mRNA and protein expression were effectively decreased (Fig. 5A, B). G9a knockdown resulted in the accumulation of cells in G0/G1, a decreased G2/M population (Fig. 5D) and nuclear accumulation of p-serine-317 Chk1 (Fig. 5F). Transcriptional changes associated to G9a gene end protein knockdown were similar to those observed in BIX-01294 treated cells, with downregulation of GLP and upregulation of p21, SOD1 and catalase (Fig. 5E). To assess whether alterations of proliferative capacity and alterations of genes controlling cell cycle by G9a HMT inhibition in endothelial cells affect tube formation abilities, we employed a matrigel assay. BIX-01294 clearly inhibited the formation of capillary-like structures by both HMEC-1 and primary HUVEC in a matrigel matrix, in accordance with a recent independent report [41]. Taken together, the data obtained from a G9a knockdown approach in HMEC-1 cells reveal a commonality of action between the chemically-induced inhibition of G9a and its transcriptional repression (as schematically represented in Fig. 7), and provide evidence that antitumorigenic actions of G9a HMT inhibitors are directed not only against cancer cells, but can also effectively work via inhibition of tumor-associated neovascularization.
Conflict of interest statement
Acknowledgements
Introduction
Members of the Set1/MLL (mixed lineage leukemia) family of methyltransferases (KMT2) catalyze the methylation of lysine 4 of histone H3 (H3K4) (Piunti and Shilatifard, 2016, Shilatifard, 2012). Conserved from yeast to human, the methyltransferase activity of these enzymes is associated with gene regulatory events that play a critical role in hematopoiesis, embryonic stem cell development, and neurogenesis (Barski et al., 2007, Ruthenburg et al., 2007, Shilatifard, 2012, Sze and Shilatifard, 2016). Misregulation of the Set1/MLL family is highly correlated with diverse pathologies (Ng et al., 2010, Singh et al., 2016, Sze et al., 2017, Wang et al., 2018), such as pediatric acute lymphocytic leukemia and adult acute myeloid leukemia, where recurrent chromosomal translocation of the MLL1 gene is frequently identified (Andersson et al., 2015, Slany, 2016, Yang and Ernst, 2017). Humans possess at least six MLL homologs with non-redundant functions (Shilatifard, 2012). In budding yeast S. cerevisiae, the one and only Set1/COMPASS (complex of proteins associated with Set1) complex is responsible for the mono-, di-, and tri-methylation of H3K4 (Bernstein et al., 2002, Briggs et al., 2001, Krogan et al., 2002, Miller et al., 2001, Nagy et al., 2002). Akin to its human homolog, the Set1 protein on its own displays weak mono-methyltransferase activity but is positively allosterically regulated upon association with a multi-subunit complex comprised of Cps30, Cps50, Cps60, and Cps25 (Takahashi et al., 2011). This specific set of core components is shared among species. For instance, the WRAD complex (WDR5/RbBP5/ASH2L/DPY30, corresponding to Cps30/50/60/25) is shared in all six MLL methyltransferases in human cells (Couture and Skiniotis, 2013), and absence of any WRAD protein compromises, to different extents, the function of MLL/COMPASS-like complexes (Avdic et al., 2011a, Dou et al., 2006, Patel et al., 2009, Steward et al., 2006, Zhang et al., 2012).
Our earlier EM studies showed the subunit organization and a similar Y-shaped architecture adopted by both core COMPASS and human MLL (Takahashi et al., 2011) but lacked the resolution to reveal structural details. On the other hand, high-resolution structures of MLL’s fragment or subunits from us and others have provided crucial insights (Avdic et al., 2011a, Couture et al., 2006, Li et al., 2016, Odho et al., 2010, Zhang et al., 2015) but do not capture the entire spectrum of interactions contributing to the formation of MLL complexes and likely hinder our understanding of hitherto unknown but potentially important regions of partner proteins regulating KMT2 enzymes. Here, we employed single-particle cryo-EM, complemented by X-ray crystallography and functional assays, to obtain a detailed structural model for the yeast S. cerevisiae COMPASS complex including Set1(726-1080 aa), Cps30, Cps50, Cps60, Cps25, and Cps40. The results highlight the essential scaffolding role of Cps50 for COMPASS assembly, the conformationally dynamic character of the complex, and the essential role of Cps30 on inducing higher methylation states of H3K4.