Extensive non-canonical phosphorylation in human cells revealed using strong-anion exchange-mediated phosphoproteomics

Hardman, Gemma; Perkins, Simon; Ruan, Zheng; Kannan, Natarajan; Brownridge, Philip; Byrne, Dominic P.; Eyers, Patrick A.; Jones, Andrew R.

doi:10.1101/202820

Cited by 11 publications

(9 citation statements)

References 86 publications

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“…Interestingly, Leu residues were globally overrepresented in the sequence motifs surrounding the three phosphoramidate bonds on His, Lys, and Arg but this was not the case when considering the phosphopeptides with phosphorylated Ser, Thr, and Tyr (data not shown). Similar observations were also made by Hardman et al 5 and might suggest selectivity for phosphoramidates bonds or a preferential adsorption to the resins used, but most probably stabilization against hydrolysis by local hydrophobic acids.…”

Section: → Strict Non-acidic Conditions Permit Purification Of Phis Csupporting

confidence: 85%

“…Phosphoramidate includes the histidine phosphorylation, welldefined in bacteria 3,4 . Regardless of the nature of their chemical linkages, the presence of the phosphate group on all nine amino acids causes an increased mass of 79.97 Da, which can be detected by MS. During phosphopeptide fragmentation, a prominent neutral loss of phosphoric acid (98 Da) is generally observed, and it has been suggested that a triplet neutral loss fingerprint could occur for specific phosphoresidues, but recently this has been called into question [5][6][7] . One of the main reasons why these phosphoramidate bond-containing phosphoamino acids, such as phosphohistidine, have remained unexplored is their instability 8,9 .…”

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confidence: 99%

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A non-acidic method using hydroxyapatite and phosphohistidine monoclonal antibodies allows enrichment of phosphopeptides containing non-conventional phosphorylations for mass spectrometry analysis

Adam

Fuhs

Meisenhelder

et al. 2019

Preprint

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Four types of phosphate-protein linkage generate nine different phosphoresidues in living organisms. Histidine phosphorylation is a long-time established but largely unexplored post-translational modification, mainly because of the acid-lability of the phosphoramidate bonds. This lability means that standard phosphoproteomic methods used for conventional phosphate esters (phospho-Ser/Thr/Tyr) must be modified to analyze proteins containing the phosphoramidate-amino acids -phospho-His/Arg/Lys. We show that a non-acidic method allows enrichment of non-conventional phosphoresiduecontaining peptides from tryptic digests of human cell lines, using hydroxyapatite binding and/or immobilized 1-pHis and 3-pHis monoclonal antibodies for enrichment. 425 unique non-conventional phosphorylation sites (i.e. pHis, pLys and pArg) were detected with a high probability of localization by LC-MS/MS analysis and identified using a customized MaxQuant configuration, contributing to a new era of study in post-translational modification and cell signaling in humans. This is the first fully non-acidic method for phosphopeptide enrichment which uses immunoaffinity purification and remains compatible with mass spectrometry analysis for a wider coverage of potential protein phosphorylation events. Introduction:Phosphoproteomics has contributed to tremendous progress in the field of life science and revealed the extensive use of phosphorylation as one of the most important post-translational modifications in eukaryotic organisms. The identification and characterization of phosphorylation sites has been revolutionized by mass spectrometry (MS) with faster and more sensitive instruments. Progress in phosphosite-mapping with tandem mass spectrometry (MS/MS) has allowed improved localization and phosphorylation assignment to a single residue with high confidence. The development of bioinformatics tools for large-scale phosphoproteome data analysis was an equally important step and permitted the integration of different parameters searching for complex combinatorial possibilities 1,2 .Up until now, only one class of phosphate-bond containing phosphoamino acid, corresponding to the conventional serine, threonine and tyrosine phosphorylation (phosphate-ester or O-phosphate) has been systematically considered for phosphorylation site searching. But nine out of the 20 amino acids have the

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Section: → Strict Non-acidic Conditions Permit Purification Of Phis Csupporting

confidence: 85%

mentioning

confidence: 99%

A non-acidic method using hydroxyapatite and phosphohistidine monoclonal antibodies allows enrichment of phosphopeptides containing non-conventional phosphorylations for mass spectrometry analysis

Adam

Fuhs

Meisenhelder

et al. 2019

Preprint

View full text Add to dashboard Cite

show abstract

“…Recent studies aimed at systematic large-scale detection of six acid-labile protein phosphorylation in human cell extracts have exposed the difficulty of confident localization of phosphate groups on Arg, His, Lys, Asp, Glu, and Cys residues. Although phosphorothiol ester linkage is moderately acid-stable and highly base-stable, protein cysteine phosphorylation was not detected in these studies (Hardman et al 2017). The lack of basic information on the prevalence, properties, and behavior of this modification under analytical circumstances explains this lack of success.…”

Section: Discussionmentioning

confidence: 85%

“…Triplet-like phosphate losses, generated by HCDfragmentation from molecular ions of pCys-peptides, are similar to the neutral-loss triplets (or missing M-116 signal NL-doublets) observed for many phosphohistidine peptides (Oslund et al 2014;Potel et al 2018a). Earlier, Hardman et al had thoroughly evaluated identification of pHis-peptides by the triplet-like loss pattern (Hardman et al 2017) and concluded that this trait was not a general hallmark of histidine phosphorylation.…”

Section: Characteristics Of Hcd-type Fragmentation Of Pcys-peptidesmentioning

confidence: 87%

Modified cysteine S-phosphopeptide standards for mass spectrometry-based proteomics

Buchowiecka

2019

Amino Acids

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The regulatory role of protein cysteine phosphorylation is an under-researched area. The difficulty of accessing reference S-phosphorylated peptides (pCys-peptides) hampers progress in MS-driven cysteine phosphoproteomics, which requires targeted analytical procedures. This work describes an uncomplicated process for the conversion of disulfide-bridged protein into a complex model mixture of combinatorially modified peptides. Hen egg-white lysozyme was reduced with tris(2carboxyethyl)phosphine (TCEP) followed by alkylation of cysteine with (3-acrylamidopropyl)trimethyl-ammonium chloride (APTA) and subsequent beta-elimination in aqueous Ba(OH) 2 to yield modified polypeptides containing multiple dehydroalanine (Dha) residues. The conjugate addition of thiophosphoric acid to Dha residues followed by trypsinolysis led to numerous D/L phosphocysteine-containing peptides, which were identified by higher-energy collisional-dissociation tandem mass spectrometry (HCD-MS/MS). Our results show that some pCys-peptides produce prominent neutral losses of 80 Da, 98 Da and a weak 116 Da loss. These are similar to the neutral-loss triplets generated by phosphohistidine peptides.

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“…[ 46 ] As another example, a high‐throughput analysis of phospho‐tyrosine has revealed a large proportion of noncanonical P‐sites. [ 51 ] All these data are in accordance with the concept that the structure of the kinase catalytic site is dynamic, and that it adapts to flexible substrates. [ 52 ] To investigate briefly this complexity, we have checked 600 protein substrates of 60 kinases representing the major families retrieved from PhosphoSitePlus and covering more than 10 000 phosphorylated sites as a limited representative panel of the full phospho landscape.…”

Section: Introductionmentioning

confidence: 99%

Protein Phosphorylation Dynamics: Unexplored Because of Current Methodological Limitations

Robichon

2020

BioEssays

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The study of intrinsic phosphorylation dynamics and kinetics in the context of complex protein architecture in vivo has been challenging: Method limitations have prevented significant advances in the understanding of the highly variable turnover of phosphate groups, synergy, and cooperativity between P‐sites. However, over the last decade, powerful analytical technologies have been developed to determine the full catalog of the phosphoproteome for many species. The curated databases of phospho sites found by mass spectrometry analysis and the computationally predicted sites based on the linear sequence of kinase motifs are valuable tools. They allow investigation of the complexity of phosphorylation in vivo, albeit with strong discrepancies between different methods. A series of hypothetical scenarios on combinatorial processive phosphorylation is proposed that are likely unverifiable with current methodologies. These proposed a priori postulates could be considered as possible extensions of the known schemes of the activation/inhibition signaling process in vivo.

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Extensive non-canonical phosphorylation in human cells revealed using strong-anion exchange-mediated phosphoproteomics

Cited by 11 publications

References 86 publications

A non-acidic method using hydroxyapatite and phosphohistidine monoclonal antibodies allows enrichment of phosphopeptides containing non-conventional phosphorylations for mass spectrometry analysis

A non-acidic method using hydroxyapatite and phosphohistidine monoclonal antibodies allows enrichment of phosphopeptides containing non-conventional phosphorylations for mass spectrometry analysis

Modified cysteine S-phosphopeptide standards for mass spectrometry-based proteomics

Protein Phosphorylation Dynamics: Unexplored Because of Current Methodological Limitations

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