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      MeCP2 post-translational modifications: a mechanism to control its involvement in synaptic plasticity and homeostasis?

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          Abstract

          Although Rett syndrome (RTT) represents one of the most frequent forms of severe intellectual disability in females worldwide, we still have an inadequate knowledge of the many roles played by MeCP2 (whose mutations are responsible for most cases of RTT) and their relevance for RTT pathobiology. Several studies support a role of MeCP2 in the regulation of synaptic plasticity and homeostasis. At the molecular level, MeCP2 is described as a repressor capable of inhibiting gene transcription through chromatin compaction. Indeed, it interacts with several chromatin remodeling factors, such as HDAC-containing complexes and ATRX. Other studies have inferred that MeCP2 functions also as an activator; a role in regulating mRNA splicing and in modulating protein synthesis has also been proposed. Further, MeCP2 avidly binds both 5-methyl- and 5-hydroxymethyl-cytosine. Recent evidence suggests that it is the highly disorganized structure of MeCP2, together with its post-translational modifications (PTMs) that generate and regulate this functional versatility. Indeed, several reports have demonstrated that differential phosphorylation of MeCP2 is a key mechanism by which the methyl binding protein modulates its affinity for its partners, gene expression and cellular adaptations to stimuli and neuronal plasticity. As logic consequence, generation of phospho-defective Mecp2 knock-in mice has permitted associating alterations in neuronal morphology, circuit formation, and mouse behavioral phenotypes with specific phosphorylation events. MeCP2 undergoes various other PTMs, including acetylation, ubiquitination and sumoylation, whose functional roles remain largely unexplored. These results, together with the genome-wide distribution of MeCP2 and its capability to substitute histone H1, recall the complex regulation of histones and suggest the relevance of quickly gaining a deeper comprehension of MeCP2 PTMs, the respective writers and readers and the consequent functional outcomes.

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          Rett syndrome is caused by mutations in X-linked MECP2, encoding methyl-CpG-binding protein 2.

          Ruthie Amir, Ignatia B Van den Veyver, Mimi Wan (1999)
          Rett syndrome (RTT, MIM 312750) is a progressive neurodevelopmental disorder and one of the most common causes of mental retardation in females, with an incidence of 1 in 10,000-15,000 (ref. 2). Patients with classic RTT appear to develop normally until 6-18 months of age, then gradually lose speech and purposeful hand use, and develop microcephaly, seizures, autism, ataxia, intermittent hyperventilation and stereotypic hand movements. After initial regression, the condition stabilizes and patients usually survive into adulthood. As RTT occurs almost exclusively in females, it has been proposed that RTT is caused by an X-linked dominant mutation with lethality in hemizygous males. Previous exclusion mapping studies using RTT families mapped the locus to Xq28 (refs 6,9,10,11). Using a systematic gene screening approach, we have identified mutations in the gene (MECP2 ) encoding X-linked methyl-CpG-binding protein 2 (MeCP2) as the cause of some cases of RTT. MeCP2 selectively binds CpG dinucleotides in the mammalian genome and mediates transcriptional repression through interaction with histone deacetylase and the corepressor SIN3A (refs 12,13). In 5 of 21 sporadic patients, we found 3 de novo missense mutations in the region encoding the highly conserved methyl-binding domain (MBD) as well as a de novo frameshift and a de novo nonsense mutation, both of which disrupt the transcription repression domain (TRD). In two affected half-sisters of a RTT family, we found segregation of an additional missense mutation not detected in their obligate carrier mother. This suggests that the mother is a germline mosaic for this mutation. Our study reports the first disease-causing mutations in RTT and points to abnormal epigenetic regulation as the mechanism underlying the pathogenesis of RTT.
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            PhosphoSitePlus: a comprehensive resource for investigating the structure and function of experimentally determined post-translational modifications in man and mouse

            Peter V. Hornbeck, Jon M. Kornhauser, Sasha Tkachev (2011)
            PhosphoSitePlus (http://www.phosphosite.org) is an open, comprehensive, manually curated and interactive resource for studying experimentally observed post-translational modifications, primarily of human and mouse proteins. It encompasses 1 30 000 non-redundant modification sites, primarily phosphorylation, ubiquitinylation and acetylation. The interface is designed for clarity and ease of navigation. From the home page, users can launch simple or complex searches and browse high-throughput data sets by disease, tissue or cell line. Searches can be restricted by specific treatments, protein types, domains, cellular components, disease, cell types, cell lines, tissue and sequences or motifs. A few clicks of the mouse will take users to substrate pages or protein pages with sites, sequences, domain diagrams and molecular visualization of side-chains known to be modified; to site pages with information about how the modified site relates to the functions of specific proteins and cellular processes and to curated information pages summarizing the details from one record. PyMOL and Chimera scripts that colorize reactive groups on residues that are modified can be downloaded. Features designed to facilitate proteomic analyses include downloads of modification sites, kinase–substrate data sets, sequence logo generators, a Cytoscape plugin and BioPAX download to enable pathway visualization of the kinase–substrate interactions in PhosphoSitePlus®.
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              Methylated DNA and MeCP2 recruit histone deacetylase to repress transcription.

              P Jones, G Veenstra, P A Wade (1998)
              CpG methylation in vertebrates correlates with alterations in chromatin structure and gene silencing. Differences in DNA-methylation status are associated with imprinting phenomena and carcinogenesis. In Xenopus laevis oocytes, DNA methylation dominantly silences transcription through the assembly of a repressive nucleosomal array. Methylated DNA assembled into chromatin binds the transcriptional repressor MeCP2 which cofractionates with Sin3 and histone deacetylase. Silencing conferred by MeCP2 and methylated DNA can be relieved by inhibition of histone deacetylase, facilitating the remodelling of chromatin and transcriptional activation. These results establish a direct causal relationship between DNA methylation-dependent transcriptional silencing and the modification of chromatin.
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                Author and article information

                Contributors
                Journal
                Journal ID (nlm-ta): Front Cell Neurosci
                Journal ID (iso-abbrev): Front Cell Neurosci
                Journal ID (publisher-id): Front. Cell. Neurosci.
                Title: Frontiers in Cellular Neuroscience
                Publisher: Frontiers Media S.A.
                ISSN (Electronic): 1662-5102
                Publication date (Electronic): 13 August 2014
                Publication date Collection: 2014
                Volume: 8
                Electronic Location Identifier: 236
                Affiliations
                [1] 1Division of Neuroscience, San Raffaele Rett Research Center, San Raffaele Scientific Institute Milan, Italy
                [2] 2Department of Biosciences, University of Milan Milan, Italy
                [3] 3Section of Biomedical Research, Laboratory of Genetic and Epigenetic Control of Gene Expression, Department of Theoretic and Applied Sciences, University of Insubria Busto Arsizio, Italy
                Author notes

                Edited by: Hansen Wang, University of Toronto, Canada

                Reviewed by: Daniela Tropea, Trinity College Dublin, Ireland; Juan Ausio, University of Victoria, Canada; Xiaoting Wang, Duke University, USA

                *Correspondence: Nicoletta Landsberger, Laboratory of Genetic and Epigenetic Control of Gene Expression, Department of Theoretic and Applied Biosciences, Via Manara 7, Busto Arsizio 21052, Italy e-mail: landsben@ 123456uninsubria.it

                This article was submitted to the journal Frontiers in Cellular Neuroscience.

                †Co-corresponding authors.

                Article
                DOI: 10.3389/fncel.2014.00236
                PMC ID: 4131190
                PubMed ID: 25165434
                SO-VID: 7caab60e-64b1-42a7-8d0c-026118108de5
                Copyright © Copyright © 2014 Bellini, Pavesi, Barbiero, Bergo, Chandola, Nawaz, Rusconi, Stefanelli, Strollo, Valente, Kilstrup-Nielsen and Landsberger.
                License:

                This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.

                History
                Date received : 13 May 2014
                Date accepted : 27 July 2014
                Page count
                Figures: 3, Tables: 2, Equations: 0, References: 111, Pages: 15, Words: 11997
                Categories
                Subject: Neuroscience
                Subject: Review Article

                ScienceOpen disciplines: Neurosciences
                Keywords: chromatin,mecp2,mouse models,phosphorylation,post-translational modifications,rett syndrome,synaptic plasticity
                Data availability:
                ScienceOpen disciplines: Neurosciences
                Keywords: chromatin, mecp2, mouse models, phosphorylation, post-translational modifications, rett syndrome, synaptic plasticity

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