Your search keyword '"Mer G"' showing total 6 results

1. TIRR regulates 53BP1 by masking its histone methyl-lysine binding function.

Author

Drané P, Brault ME, Cui G, Meghani K, Chaubey S, Detappe A, Parnandi N, He Y, Zheng XF, Botuyan MV, Kalousi A, Yewdell WT, Münch C, Harper JW, Chaudhuri J, Soutoglou E, Mer G, and Chowdhury D

Subjects

Animals, Ataxia Telangiectasia Mutated Proteins metabolism, Binding Sites, DNA Breaks, Double-Stranded, DNA Repair, Female, Humans, Methylation, Mice, Mice, Inbred C57BL, Phosphorylation, Protein Binding, Protein Domains, RNA-Binding Proteins, Telomere-Binding Proteins metabolism, Tumor Suppressor p53-Binding Protein 1 chemistry, Carrier Proteins metabolism, Histones chemistry, Histones metabolism, Lysine metabolism, Tumor Suppressor p53-Binding Protein 1 antagonists & inhibitors, Tumor Suppressor p53-Binding Protein 1 metabolism

Abstract

P53-binding protein 1 (53BP1) is a multi-functional double-strand break repair protein that is essential for class switch recombination in B lymphocytes and for sensitizing BRCA1-deficient tumours to poly-ADP-ribose polymerase-1 (PARP) inhibitors. Central to all 53BP1 activities is its recruitment to double-strand breaks via the interaction of the tandem Tudor domain with dimethylated lysine 20 of histone H4 (H4K20me2). Here we identify an uncharacterized protein, Tudor interacting repair regulator (TIRR), that directly binds the tandem Tudor domain and masks its H4K20me2 binding motif. Upon DNA damage, the protein kinase ataxia-telangiectasia mutated (ATM) phosphorylates 53BP1 and recruits RAP1-interacting factor 1 (RIF1) to dissociate the 53BP1-TIRR complex. However, overexpression of TIRR impedes 53BP1 function by blocking its localization to double-strand breaks. Depletion of TIRR destabilizes 53BP1 in the nuclear-soluble fraction and alters the double-strand break-induced protein complex centring 53BP1. These findings identify TIRR as a new factor that influences double-strand break repair using a unique mechanism of masking the histone methyl-lysine binding function of 53BP1.

Published

2017

2. Identification of a fragment-like small molecule ligand for the methyl-lysine binding protein, 53BP1.

Author

Perfetti MT, Baughman BM, Dickson BM, Mu Y, Cui G, Mader P, Dong A, Norris JL, Rothbart SB, Strahl BD, Brown PJ, Janzen WP, Arrowsmith CH, Mer G, McBride KM, James LI, and Frye SV

Subjects

Animals, B-Lymphocytes drug effects, Benzamides chemistry, Benzamides pharmacology, Binding Sites, Chromatin metabolism, Crystallography, X-Ray, Diamines chemistry, Diamines pharmacology, HEK293 Cells, Histones genetics, Histones metabolism, Humans, Ligands, Magnetic Resonance Spectroscopy, Mice, Inbred C57BL, Protein Structure, Tertiary, Small Molecule Libraries chemistry, Small Molecule Libraries metabolism, Structure-Activity Relationship, Tumor Suppressor p53-Binding Protein 1, Benzamides metabolism, Diamines metabolism, Intracellular Signaling Peptides and Proteins chemistry, Intracellular Signaling Peptides and Proteins metabolism, Lysine metabolism

Abstract

Improving our understanding of the role of chromatin regulators in the initiation, development, and suppression of cancer and other devastating diseases is critical, as they are integral players in regulating DNA integrity and gene expression. Developing small molecule inhibitors for this target class with cellular activity is a crucial step toward elucidating their specific functions. We specifically targeted the DNA damage response protein, 53BP1, which uses its tandem tudor domain to recognize histone H4 dimethylated on lysine 20 (H4K20me2), a modification related to double-strand DNA breaks. Through a cross-screening approach, we identified UNC2170 (1) as a micromolar ligand of 53BP1, which demonstrates at least 17-fold selectivity for 53BP1 as compared to other methyl-lysine (Kme) binding proteins tested. Structural studies revealed that the tert-butyl amine of UNC2170 anchors the compound in the methyl-lysine (Kme) binding pocket of 53BP1, making it competitive with endogenous Kme substrates. X-ray crystallography also demonstrated that UNC2170 binds at the interface of two tudor domains of a 53BP1 dimer. Importantly, this compound functions as a 53BP1 antagonist in cellular lysates and shows cellular activity by suppressing class switch recombination, a process which requires a functional 53BP1 tudor domain. These results demonstrate that UNC2170 is a functionally active, fragment-like ligand for 53BP1.

Published

2015

3. Structural plasticity of methyllysine recognition by the tandem tudor domain of 53BP1.

Author

Tong Q, Cui G, Botuyan MV, Rothbart SB, Hayashi R, Musselman CA, Singh N, Appella E, Strahl BD, Mer G, and Kutateladze TG

Subjects

Amino Acid Sequence, Humans, Intracellular Signaling Peptides and Proteins metabolism, Magnetic Resonance Spectroscopy, Molecular Sequence Data, Multiprotein Complexes metabolism, Protein Structure, Tertiary, Tumor Suppressor p53-Binding Protein 1, DNA Methylation physiology, Intracellular Signaling Peptides and Proteins chemistry, Lysine metabolism, Models, Molecular, Multiprotein Complexes chemistry

Abstract

p53 is dynamically regulated through various posttranslational modifications (PTMs), which differentially modulate its function and stability. The dimethylated marks p53K370me2 and p53K382me2 are associated with p53 activation or stabilization and both are recognized by the tandem Tudor domain (TTD) of 53BP1, a p53 cofactor. Here we detail the molecular mechanisms for the recognition of p53K370me2 and p53K382me2 by 53BP1. The solution structures of TTD in complex with the p53K370me2 and p53K382me2 peptides show a remarkable plasticity of 53BP1 in accommodating these diverse dimethyllysine-containing sequences. We demonstrate that dimeric TTDs are capable of interacting with the two PTMs on a single p53K370me2K382me2 peptide, greatly strengthening the 53BP1-p53 interaction. Analysis of binding affinities of TTD toward methylated p53 and histones reveals strong preference of 53BP1 for p53K382me2, H4K20me2, and H3K36me2 and suggests a possible role of multivalent contacts of 53BP1 in p53 targeting to and accumulation at the sites of DNA damage., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

4. PHF20 is an effector protein of p53 double lysine methylation that stabilizes and activates p53.

Author

Cui G, Park S, Badeaux AI, Kim D, Lee J, Thompson JR, Yan F, Kaneko S, Yuan Z, Botuyan MV, Bedford MT, Cheng JQ, and Mer G

Subjects

Antigens, Neoplasm genetics, Biomarkers, Tumor genetics, Cell Line, Cell Line, Tumor, Crystallography, X-Ray, DNA Damage, DNA-Binding Proteins, Gene Knockdown Techniques, Humans, Lysine chemistry, Methylation, Models, Molecular, Protein Multimerization, Protein Stability, Protein Structure, Tertiary, Transcription Factors, Tumor Suppressor Protein p53 chemistry, Tumor Suppressor Protein p53 genetics, Ubiquitination, Up-Regulation, Antigens, Neoplasm chemistry, Antigens, Neoplasm metabolism, Biomarkers, Tumor chemistry, Biomarkers, Tumor metabolism, Lysine metabolism, Tumor Suppressor Protein p53 metabolism

Abstract

PHF20 is a multidomain protein and subunit of a lysine acetyltransferase complex that acetylates histone H4 and p53 but whose function is unclear. Using biochemical, biophysical and cellular approaches, we determined that PHF20 is a direct regulator of p53. A Tudor domain in PHF20 recognized p53 dimethylated at Lys370 or Lys382 and a homodimeric form of this Tudor domain could associate with the two dimethylated sites on p53 with enhanced affinity, indicating a multivalent interaction. Association with PHF20 promotes stabilization and activation of p53 by diminishing Mdm2-mediated p53 ubiquitylation and degradation. PHF20 contributes to upregulation of p53 in response to DNA damage, and ectopic expression of PHF20 in different cell lines leads to phenotypic changes that are hallmarks of p53 activation. Overall our work establishes that PHF20 functions as an effector of p53 methylation that stabilizes and activates p53.

Published

2012

5. Preparation of recombinant peptides with site- and degree-specific lysine (13)C-methylation.

Author

Cui G, Botuyan MV, and Mer G

Subjects

Chromatography, Liquid, Methylation, Nuclear Magnetic Resonance, Biomolecular, Peptides isolation & purification, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Carbon Isotopes chemistry, Lysine metabolism, Peptides metabolism

Abstract

Lysine methylation is an important post-translational modification that affects protein function; for example, the transcriptional activity of the p53 tumor suppressor protein. To facilitate structural characterization of complexes involving proteins and methylated targets by nuclear magnetic resonance spectroscopy, we devised a simple method for preparing recombinant (15)N/(13)C-enriched peptides with a (13)C-methyl-labeled methylated lysine analogue. The method, which relies on the synthesis of (13)C-enriched alkylating agents, was applied to the production of 15-residue p53 peptides variously methylated at lysine analogue 370. The peptides were used to probe the methylation state-dependent interactions of mono, di, and trimethylated p53 with three different proteins.

Published

2009

6. Structural Basis for the Methylation State-Specific Recognition of Histone H4-K20 by 53BP1 and Crb2 in DNA Repair

Author

Mer, G

Published

2006