Post-translational modifications of histones H3 and H4 associated with the histone methyltransferases Suv39h1 and G9a

Robin, Philippe; Fritsch, Lauriane; Philipot, Ophélie; Svinarchuk, Fédor; Ait‐Si‐Ali, Slimane

doi:10.1186/gb-2007-8-12-r270

Cited by 35 publications

(46 citation statements)

References 58 publications

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“…27. The transgenes were tagged with double hemagglutinin (HA) and double FLAG epitopes at the N terminus as described in Ref.…”

Section: Methodsmentioning

confidence: 99%

“…The transgenes were tagged with double hemagglutinin (HA) and double FLAG epitopes at the N terminus as described in Ref. 27. HeLa and C2C12 control cell lines transduced with the empty vector were also established.…”

Section: Methodsmentioning

confidence: 99%

“…1A) from chromatin enriched in mononucleosomes (as described in Ref. 27). Mass spectrometry analysis of MyoD complex confirmed some "historical" partners of MyoD such as Id, E12/E47, and MEIS1, and other partners that have never been described to interact with MyoD, among them HP1 proteins, as confirmed by Western blotting (Fig.…”

Section: Hp1 Proteinsmentioning

confidence: 99%

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Differential Cooperation between Heterochromatin Protein HP1 Isoforms and MyoD in Myoblasts

Yahi

Fritsch

Philipot

et al. 2008

Journal of Biological Chemistry

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Mechanisms of transcriptional repression are important during cell differentiation. Mammalian heterochromatin protein 1 isoforms HP1␣, HP1␤, and HP1␥ play important roles in the regulation of chromatin structure and function. We explored the possibility of different roles for the three HP1 isoforms in an integrated system, skeletal muscle terminal differentiation. In this system, terminal differentiation is initiated by the transcription factor MyoD, whose target genes remain mainly silent until myoblasts are induced to differentiate. Here we show that HP1␣ and HP1␤ isoforms, but not HP1␥, interact with MyoD in myoblasts. This interaction is direct, as shown using recombinant proteins in vitro. A gene reporter assay revealed that HP1␣ and HP1␤, but not HP1␥, inhibit MyoD transcriptional activity, suggesting a model in which MyoD could serve as a bridge between nucleosomes and chromatin-binding proteins such as HDACs and HP1. Chromatin immunoprecipitation assays show a preferential recruitment of HP1 proteins on MyoD target genes in proliferating myoblasts. Finally, modulation of HP1 protein level impairs MyoD target gene expression and muscle terminal differentiation. Together, our data show a nonconventional interaction between HP1 and a tissue-specific transcription factor, MyoD. In addition, they strongly suggest that HP1 isoforms play important roles during muscle terminal differentiation in an isoform-dependent manner.

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“…27. The transgenes were tagged with double hemagglutinin (HA) and double FLAG epitopes at the N terminus as described in Ref.…”

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Differential Cooperation between Heterochromatin Protein HP1 Isoforms and MyoD in Myoblasts

Yahi

Fritsch

Philipot

et al. 2008

Journal of Biological Chemistry

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“…In the majority of these studies, a relative abundance strategy was applied (8,13,14,18,19): histones were extracted from two or more biological samples and processed in parallel. The relative percentage, rather than the absolute amount of one or more particular histone PTMs, is quantified and compared.…”

mentioning

confidence: 99%

“…This bias would potentially cause problems in the interpretation of histone PTM data, especially when there is a need for absolute quantification. It would also cause a problem for relative quantifications-because the data are normalized to the total signal from all isoforms of a peptide (8,13,14,18,19), bias in quantification of one particular form would affect all the other forms. To overcome these issues, we present here a library of 93 synthetic histone peptides and comprehensive analyses of these peptides using bottom-up nano-LC-MS/MS and correction factors generated through normalization of their detection efficiencies.…”

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confidence: 99%

Stable-isotope-labeled Histone Peptide Library for Histone Post-translational Modification and Variant Quantification by Mass Spectrometry

Lin

Wein

Gonzales-Cope

et al. 2014

Molecular & Cellular Proteomics

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To facilitate accurate histone variant and post-translational modification (PTM) quantification via mass spectrometry, we present a library of 93 synthetic peptides using Protein-Aqua™ technology. The library contains 55 peptides representing different modified forms from histone H3 peptides, 23 peptides representing H4 peptides, 5 peptides representing canonical H2A peptides, 8 peptides representing H2A.Z peptides, and peptides for both macroH2A and H2A.X. The PTMs on these peptides include lysine mono-(me1), di-(me2), and tri-methylation (me3); lysine acetylation; arginine me1; serine/threonine phosphorylation; and N-terminal acetylation. The library was subjected to chemical derivatization with propionic anhydride, a widely employed protocol for histone peptide quantification. Subsequently, the detection efficiencies were quantified using mass spectrometry extracted ion chromatograms. The library yields a wide spectrum of detection efficiencies, with more than 1700-fold difference between the peptides with the lowest and highest efficiencies. In this paper, we describe the impact of different modifications on peptide detection efficiencies and provide a resource to correct for detection biases among the 93 histone peptides. In brief, there is no correlation between detection efficiency and molecular weight, hydrophobicity, basicity, or modification type. The same types of modifications may have very different effects on detection efficiencies depending on their positions within a peptide. We also observed antagonistic effects between modifications. In a study of mouse trophoblast stem cells, we utilized the detection efficiencies of the peptide library to correct for histone PTM/variant quantification. For most histone peptides examined, the corrected data did not change the biological conclusions but did alter the relative abundance of these peptides. For a low-abundant histone H2A variant, macroH2A, the corrected data led to a different conclusion than the uncorrected data. The peptide library and detection efficiencies presented here may serve as a resource to facilitate studies in the epigenetics and proteomics fields. In eukaryotes, histones package and order DNA into nucleosomes. Histones are critical for the structural organization and transcriptional activities of chromatin. These proteins are highly conserved in eukaryotes, but they have very dynamic functions and are subject to many different regulatory mechanisms (1). One of the major mechanisms is enacted via the use of different histone variants and post-translational modifications (PTMs). 1Over the past two decades, accumulating evidence has suggested that levels and PTM compositions of many histone variants play important roles in cellular processes and human diseases. There are increasing needs for the precise quantification of histone variants and PTMs in biomedical studies. Mass spectrometry (MS) has proved to be a robust and powerful tool for analyzing histones, as it can be used to simultaneously identify and quantify histone variants and ...

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Drawbacks in the use of unconventional hydrophobic anhydrides for histone derivatization in bottom-up proteomics PTM analysis

et al. 2015

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Mass spectrometry (MS)-based proteomics has become the most utilized tool to characterize histone post-translational modifications (PTMs). Since histones are highly enriched in lysine and arginine residues, lysine derivatization has been developed to prevent the generation of short peptides (3-6 residues) during trypsin digestion. One of the most adopted protocols applies propionic anhydride for derivatization. However, the propionyl group is not sufficiently hydrophobic to fully retain the shortest histone peptides in reversed-phase liquid chromatography, and such procedure also hampers the discovery of natural propionylation events. In this work we tested 12 commercially available anhydrides, selected based on their safety and hydrophobicity. Performance was evaluated in terms of yield of the reaction, MS/MS fragmentation efficiency and drift in retention time by using the following samples: (i) a synthetic unmodified histone H3 tail, (ii) synthetic modified histone peptides and (iii) a histone extract from cell lysate. Results highlighted that 7 of the selected anhydrides increased peptide retention time as compared to propionic, and several anhydrides such as benzoic and valeric led to high MS/MS spectra quality. However, propionic anhydride derivatization still resulted in our opinion as the best protocol to achieve high MS sensitivity and more even ionization efficiency among the analyzed peptides.

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Post-translational modifications of histones H3 and H4 associated with the histone methyltransferases Suv39h1 and G9a

Cited by 35 publications

References 58 publications

Differential Cooperation between Heterochromatin Protein HP1 Isoforms and MyoD in Myoblasts

Differential Cooperation between Heterochromatin Protein HP1 Isoforms and MyoD in Myoblasts

Stable-isotope-labeled Histone Peptide Library for Histone Post-translational Modification and Variant Quantification by Mass Spectrometry

Drawbacks in the use of unconventional hydrophobic anhydrides for histone derivatization in bottom-up proteomics PTM analysis

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