Structural Basis of LSD1-CoREST Selectivity in Histone H3 Recognition

Forneris, Federico; Binda, Claudia; Adamo, Antonio; Battaglioli, Elena; Mattevi, Andrea

doi:10.1074/jbc.c700100200

Cited by 213 publications

(352 citation statements)

References 22 publications

(48 reference statements)

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“…6(E)]. 70 A substrate-like peptide was generated by a K5M mutation (marked in gray in Fig. 6) because this mutation led to 30-fold increase in binding affinity thereby helping to stabilize the complex.…”

Section: Examination Of the Morfs In Rnap II And Histone H3mentioning

confidence: 99%

Exploring the binding diversity of intrinsically disordered proteins involved in one‐to‐many binding

et al. 2013

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Molecular recognition features (MoRFs) are intrinsically disordered protein regions that bind to partners via disorder-to-order transitions. In one-to-many binding, a single MoRF binds to two or more different partners individually. MoRF-based one-to-many protein-protein interaction (PPI) examples were collected from the Protein Data Bank, yielding 23 MoRFs bound to 2-9 partners, with all pairs of same-MoRF partners having less than 25% sequence identity. Of these, 8 MoRFs were bound to 2-9 partners having completely different folds, whereas 15 MoRFs were bound to 2-5 partners having the same folds but with low sequence identities. For both types of partner variation, backbone and side chain torsion angle rotations were used to bring about the conformational changes needed to enable close fits between a single MoRF and distinct partners. Alternative splicing events (ASEs) and posttranslational modifications (PTMs) were also found to contribute to distinct partner binding. Because ASEs and PTMs both commonly occur in disordered regions, and because both ASEs and PTMs are often tissue-specific, these data suggest that MoRFs, ASEs, and PTMs may collaborate to alter PPI networks in different cell types. These data enlarge the set of carefully studied MoRFs that use inherent flexibility and that also use ASE-based and/or PTM-based surface modifications to enable the same disordered segment to selectively associate with two or more partners. The small number of residues involved in MoRFs and in their modifications by ASEs or PTMs may simplify the evolvability of signaling network diversity.

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Section: Examination Of the Morfs In Rnap II And Histone H3mentioning

confidence: 99%

Exploring the binding diversity of intrinsically disordered proteins involved in one‐to‐many binding

et al. 2013

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“…Some of them can remove methyl groups from two different lysine residues and, therefore, are dual-specificity histone demethylases. The crystal structure of LSD1 has been solved [38,[40][41][42] and the molecular determination for the sequence and methylation-state specificity has been uncovered. Although the structure of JMJD2A has been solved in apo form or in complex with its substrates [24][25][26][27], which provides insights into the molecular npg mechanism of catalysis and substrate recognition, how substrate specificity is determined for all other members of the JmjC domain-containing histone lysine demethylases remains to be elucidated.…”

Section: Discussionmentioning

confidence: 99%

“…Consistently, the H3K4me2 demethylase LSD1 also has a shallow active site, even though it uses a different enzymatic mechanism, and its active site shares no sequence similarity to ceKDM7A and other JmjC domain-containing proteins. In the LSD1 complex with H3 peptide analog (K4 is replaced by Met) [38], the distance between Cα and the reactive N-5 of flavin is 7.69 Å ( Figure 6B and Supplementary information, Figure S7). On the contrary, H3K9me3 and H3K36me3 demethylase JMJD2A has a large active site.…”

Section: Substrate Specificitymentioning

confidence: 99%

Structural insights into a dual-specificity histone demethylase ceKDM7A from Caenorhabditis elegans

Yang

Wang

et al. 2010

Cell Res

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Histone lysine methylation can be removed by JmjC domain-containing proteins in a sequence-and methylationstate-specific manner. However, how substrate specificity is determined and how the enzymes are regulated were largely unknown. We recently found that ceKDM7A, a PHD-and JmjC domain-containing protein, is a histone demethylase specific for H3K9me2 and H3K27me2, and the PHD finger binding to H3K4me3 guides the demethylation activity in vivo. To provide structural insight into the molecular mechanisms for the enzymatic activity and the function of the PHD finger, we solved six crystal structures of the enzyme in apo form and in complex with single or two peptides containing various combinations of H3K4me3, H3K9me2, and H3K27me2 modifications. The structures indicate that H3K9me2 and H3K27me2 interact with ceKDM7A in a similar fashion, and that the peptide-binding specificity is determined by a network of specific interactions. The geometrical measurement of the structures also revealed that H3K4me3 associated with the PHD finger and H3K9me2 bound to the JmjC domain are from two separate molecules, suggesting a trans-histone peptide-binding mechanism. Thus, our systemic structural studies reveal not only the substrate recognition by the catalytic domain but also more importantly, the molecular mechanism of dual specificity of ceDKM7A for both H3K9me2 and H3K27me2.

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“…Finally, on deprotection with trifluoroacetic acid, 3-guanidine phenyl oxazole derivatives 9 were obtained. 26 A number of N-substituted derivatives (10)(11)(12)(13)(14) were also prepared via N-acylation, N-sulfonation or N-alkylation of 6b (Scheme 2). All synthesized compounds were fully characterized by spectroscopic methods (NMR, IR, MS and HRMS).…”

Section: Communicationmentioning

confidence: 99%

“…Using the available X-ray diffraction crystal structure of LSD1 as a starting point, 14 we designed a series of small molecules as potential inhibitors taking the key pharmacophore features identified for the MAO, the polyamine/guanidine and methionine based peptide inhibitors, into account ( Fig. 1) 12,13,15-20 being linked through an oxazole moiety.…”

mentioning

confidence: 99%

Synthesis and evaluation of 3-amino/guanidine substituted phenyl oxazoles as a novel class of LSD1 inhibitors with anti-proliferative properties

et al. 2013

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A series of functionalized phenyl oxazole derivatives was designed, synthesized and screened in vitro for their activities against LSD1 and for effects on viability of cervical and breast cancer cells, and in vivo for effects using zebrafish embryos. These compounds are likely to act via multiple epigenetic mechanisms specific to cancer cells including LSD1 inhibition.Histones are proteins that bind to DNA and facilitate efficient 'packing' of DNA in eukaryotic cells. 1 They are highly basic in nature due to the presence of positively charged amino acid side chains causing the DNA to fold around them into compact structures (nucleosomes). The ability of histones to regulate gene expression is controlled by post-translational modifications on the N-terminal (and likely C-terminal) "tails" of the core histones which project out of the nucleosome. Modifications including phosphorylation, acetylation, methylation, ubiquitination, sumoylation and biotinylation have been identified on the histone tails. 2 The cellular roles of histone lysine acetylation/deacetylation are the best characterized of the histone modifications -acetylation normally activates transcription whereas deacetylation deactivates this process. 3 Although there are clear links to disease, 4-8 the role of histone methylation is much less understood and appears to be context dependent.LSD1 (lysine specific demethylase 1) was the first histone demethylase identified. Its discovery significantly advanced the understanding of epigenetic regulation of gene expression, changing the paradigm that methylation is a non-reversible feature of histones. 9 Histone methylation/demethylation has since been found to be an important epigenetic modification linked to activation as well as repression of transcription. Two types of histone demethylases have been discovered. The flavin-dependent demethylase LSD1 acts on lysine 4 and lysine 9 of histone H3 (H3K4 and H3K9). LSD1 selectively catalyzes the oxidation of the methyl group of mono-and dimethylated lysines resulting in an imine intermediate and generation of hydrogen peroxide. The imine product is non-enzymatically hydrolysed to generate a carbinolamine resulting in demethylated lysine and formaldehyde release. 10 The other major class, i.e. Jumonji domain-containing histone demethylases, are Fe(II) and 2-oxoglutarate dependent oxygenases that act on mono-, di-and trimethylated Lys and methylated Arg residues depending on the particular enzymes. 11 Histone demethylase activity is associated with several pathological states. Increased LSD1 expression in prostate tumors correlates significantly with relapse during therapy. 6,7 Suppressed LSD1 expression is associated with vascular smooth muscle cell inflammatory damage in a mouse model of diabetes. 8 Demethylation of p53 (tumor suppressor) by LSD1 prevents p53 interaction with its co-activator 53BP1. 5 Activation of the telomerase reverse transcriptase (hTERT) gene is known to be dependent on LSD1 levels and recruitment to the hTERT promoter. 4 Studies on LSD1 hav...

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Structural Basis of LSD1-CoREST Selectivity in Histone H3 Recognition

Cited by 213 publications

References 22 publications

Exploring the binding diversity of intrinsically disordered proteins involved in one‐to‐many binding

Exploring the binding diversity of intrinsically disordered proteins involved in one‐to‐many binding

Structural insights into a dual-specificity histone demethylase ceKDM7A from Caenorhabditis elegans

Synthesis and evaluation of 3-amino/guanidine substituted phenyl oxazoles as a novel class of LSD1 inhibitors with anti-proliferative properties

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