Large Scale Mass Spectrometry-based Identifications of Enzyme-mediated Protein Methylation Are Subject to High False Discovery Rates

Hart‐Smith, Gene; Yagoub, Daniel; Tay, Aidan P.; Pickford, Russell; Wilkins, Marc R.

doi:10.1074/mcp.m115.055384

Cited by 71 publications

(100 citation statements)

References 58 publications

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“…There are currently 1324 proteins with lysine methylation appearing the PhosphoSitePlus database (www.phosphosite.org) (Hornbeck et al 2012). It is important to be aware that of factors that cause high-throughput identification of methylated residues to be subject to a higher rate of false positives than other posttranslational modifications (Hart-Smith et al 2015). This is largely because of the fact that several pairs of amino acid substitutions introduce the same 14 Da mass shift as methylation (for example, glycine to alanine).…”

Section: Concluding Remarks: Understanding Lysine Methylation Across mentioning

confidence: 99%

Nonhistone Lysine Methylation in the Regulation of Cancer Pathways

Carlson

Gozani

2016

Cold Spring Harb Perspect Med

104

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Proteins are regulated by an incredible array of posttranslational modifications (PTMs). Methylation of lysine residues on histone proteins is a PTM with well-established roles in regulating chromatin and epigenetic processes. The recent discovery that hundreds and likely thousands of nonhistone proteins are also methylated at lysine has opened a tremendous new area of research. Major cellular pathways involved in cancer, such as growth signaling and the DNA damage response, are regulated by lysine methylation. Although the field has developed quickly in recent years many fundamental questions remain to be addressed. We review the history and molecular functions of lysine methylation. We then discuss the enzymes that catalyze methylation of lysine residues, the enzymes that remove lysine methylation, and the cancer pathways known tobe regulated by lysine methylation. The rest of the article focuses on two open questions that we suggest as a roadmap for future research. First is understanding the large number of candidate methyltransferase and demethylation enzymes whose enzymatic activity is not yet defined and which are potentially associated with cancer through genetic studies. Second is investigating the biological processes and cancer mechanisms potentially regulated by the multitude of lysine methylation sites that have been recently discovered.

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Section: Concluding Remarks: Understanding Lysine Methylation Across mentioning

confidence: 99%

Nonhistone Lysine Methylation in the Regulation of Cancer Pathways

Carlson

Gozani

2016

Cold Spring Harb Perspect Med

104

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“…We used protein tandem mass spectrometry (MS/MS) to identify Lys‐methylated proteins whose expression is modulated by Cd. The identification of Lys‐methylated peptides by MS/MS is still challenging for many reasons (Wang, Wang, & Ye, ), including the low abundance and/or low methylation level of targets and the high false discovery rates for methylpeptides identification due to amino acid substitutions that are isobaric with methylation events (Hart‐Smith, Yagoub, Tay, Pickford, & Wilkins, ; Ong, Mittler, & Mann, ). To address this challenge, we focused on the identification of the abundant doublet of trimethylated proteins at 26–28 kDa for which the expression pattern was potentially interesting regarding Cd stress (Figure ).…”

Section: Resultsmentioning

confidence: 99%

Protein lysine methylation contributes to modulating the response of sensitive and tolerant Arabidopsis species to cadmium stress

Serre

Sarthou

Gigarel

et al. 2019

Plant Cell & Environment

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The mechanisms underlying the response and adaptation of plants to excess of trace elements are not fully described. Here, we analysed the importance of protein lysine methylation for plants to cope with cadmium. We analysed the effect of cadmium on lysine‐methylated proteins and protein lysine methyltransferases (KMTs) in two cadmium‐sensitive species, Arabidopsis thaliana and A. lyrata, and in three populations of A. halleri with contrasting cadmium accumulation and tolerance traits. We showed that some proteins are differentially methylated at lysine residues in response to Cd and that a few genes coding KMTs are regulated by cadmium. Also, we showed that 9 out of 23 A. thaliana mutants disrupted in KMT genes have a tolerance to cadmium that is significantly different from that of wild‐type seedlings. We further characterized two of these mutants, one was knocked out in the calmodulin lysine methyltransferase gene and displayed increased tolerance to cadmium, and the other was interrupted in a KMT gene of unknown function and showed a decreased capacity to cope with cadmium. Together, our results showed that lysine methylation of non‐histone proteins is impacted by cadmium and that several methylation events are important for modulating the response of Arabidopsis plants to cadmium stress.

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“…The methods used here were different to the ones described by Hart-Smith [57] and the results were validated in the absence of alcohol-based staining. Furthermore, bacterially expressed tubulin β (which lacks methylation, Sigma; Cat#SRP5148) analysed from stained or unstained protocols, did not yield any falsely identified methylated arginine residues using the mass spectrometry protocol described above.…”

Section: Methodsmentioning

confidence: 99%

Root morphogenic pathways in Eucalyptus grandis are modified by the activity of protein arginine methyltransferases

et al. 2017

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BackgroundMethylation of proteins at arginine residues, catalysed by members of the protein arginine methyltransferase (PRMT) family, is crucial for the regulation of gene transcription and for protein function in eukaryotic organisms. Inhibition of the activity of PRMTs in annual model plants has demonstrated wide-ranging involvement of PRMTs in key plant developmental processes, however, PRMTs have not been characterised or studied in long-lived tree species.ResultsTaking advantage of the recently available genome for Eucalyptus grandis, we demonstrate that most of the major plant PRMTs are conserved in E. grandis as compared to annual plants and that they are expressed in all major plant tissues. Proteomic and transcriptomic analysis in roots suggest that the PRMTs of E. grandis control a number of regulatory proteins and genes related to signalling during cellular/root growth and morphogenesis. We demonstrate here, using chemical inhibition of methylation and transgenic approaches, that plant type I PRMTs are necessary for normal root growth and branching in E. grandis. We further show that EgPRMT1 has a key role in root hair initiation and elongation and is involved in the methylation of β-tubulin, a key protein in cytoskeleton formation.ConclusionsTogether, our data demonstrate that PRMTs encoded by E. grandis methylate a number of key proteins and alter the transcription of a variety of genes involved in developmental processes. Appropriate levels of expression of type I PRMTs are necessary for the proper growth and development of E. grandis roots. Electronic supplementary materialThe online version of this article (doi:10.1186/s12870-017-1010-x) contains supplementary material, which is available to authorized users.

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Large Scale Mass Spectrometry-based Identifications of Enzyme-mediated Protein Methylation Are Subject to High False Discovery Rates

Cited by 71 publications

References 58 publications

Nonhistone Lysine Methylation in the Regulation of Cancer Pathways

Nonhistone Lysine Methylation in the Regulation of Cancer Pathways

Protein lysine methylation contributes to modulating the response of sensitive and tolerant Arabidopsis species to cadmium stress

Root morphogenic pathways in Eucalyptus grandis are modified by the activity of protein arginine methyltransferases

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