A global atlas of substrate specificities for the human serine/threonine kinome

Johnson, Jared L.; Yaron, Tomer M.; Huntsman, Emily; Kerelsky, Alexander; Song, Junho; Regev, Amit; Lin, Ting‐Yu; Liberatore, Katarina; Cizin, Daniel M.; Cohen, Benjamin M; Vasan, Neil; Ma, Yilun; Krismer, Konstantin; Robles, Jaylissa Torres; Kooij, Bert van de; Vlimmeren, Anne E van; Andrée-Busch, Nicole; Käufer, Norbert F.; Dorovkov, Maxim V.; Ryazanov, Alexey G.; Takagi, Yuichiro; Kastenhuber, Edward R.; Goncalves, Marcus D.; Elemento, Olivier; Taatjes, Dylan J.; Maucuer, Alexandre; Yamashita, Akio; Degterev, Alexei; Linding, Rune; Blenis, John; Hornbeck, Peter; Turk, Benjamin E.; Yaffe, Michael B.; Cantley, Lewis C.

doi:10.1101/2022.05.22.492882

Cited by 20 publications

(29 citation statements)

References 108 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…If so, this would be a potentially powerful tool for the identification of native substrates and the dissection of phosphotyrosine signaling pathways. Indeed, oriented peptide libraries have been applied extensively to predict the native substrates of protein kinases (Johnson et al, 2022; Miller et al, 2008; Obenauer et al, 2003). We are particularly interested in using high-throughput specificity screens to predict how mutations proximal to phosphorylation sites affect tyrosine kinase selectivity.…”

Section: Resultsmentioning

confidence: 99%

“…The specificity profiling screens described thus far were constrained to sequences that contain the canonical twenty amino acids. Several studies have suggested that non-canonical amino acids and post-translationally modified amino acids can also impact sequence recognition by tyrosine kinases and SH2 domains (Alfaro-Lopez et al, 1998; Begley et al, 2015; Chapelat et al, 2012; Johnson et al, 2022; Yeh et al, 2001). The most notable example of this is phospho-priming, whereby phosphorylation of one residue on a protein enhances the ability of a kinase to recognize and phosphorylate a proximal residue.…”

Section: Resultsmentioning

confidence: 99%

“…Several variations on this technique have been reported to improve the throughput and quantification of sequence preferences (Deng et al, 2014; Huang et al, 2008; Hutti et al, 2004; Mok et al, 2010). Notably, this method is also applicable to serine/threonine kinases, and large swaths of the yeast and human kinomes have been characterized using oriented peptide libraries, providing significant insights into kinase-substrate recognition and phospho-signaling (Deng et al, 2014; Johnson et al, 2022; Mok et al, 2010; Songyang et al, 1995). Oriented peptide library screens have primarily been useful for determining the preference for each amino acid at a given position, independent of sequence context, but evidence suggests that some amino acid preferences may depend on the surrounding sequence (Cantor et al, 2018).…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

High-throughput profiling of sequence recognition by tyrosine kinases and SH2 domains using bacterial peptide display

Voleti

Lee

et al. 2022

Preprint

View full text Add to dashboard Cite

Tyrosine kinases and SH2 (phosphotyrosine recognition) domains have binding specificities that depend on the amino acid sequence surrounding the target (phospho)tyrosine residue. Although the preferred recognition motifs of many kinases and SH2 domains are known, we lack a quantitative description of sequence specificity that could guide predictions about signaling pathways or be used to design sequences for biomedical applications. Here, we present a platform that combines genetically-encoded peptide libraries and deep sequencing to profile sequence recognition by tyrosine kinases and SH2 domains. We screened several tyrosine kinases against a million-peptide random library and used the resulting profiles to design high-activity sequences. We also screened several kinases against a library containing thousands of human proteome-derived peptides and their naturally-occurring variants. These screens recapitulated independently measured phosphorylation rates and revealed hundreds of phosphosite-proximal mutations that impact phosphosite recognition by tyrosine kinases. We extended this platform to the analysis of SH2 domains and showed that screens could predict relative binding affinities. Finally, we expanded our method to assess the impact of non-canonical and post-translationally modified amino acids on sequence recognition. This specificity profiling platform will shed new light on phosphotyrosine signaling and could readily be adapted to other protein modification/recognition domains.

show abstract

Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

High-throughput profiling of sequence recognition by tyrosine kinases and SH2 domains using bacterial peptide display

Voleti

Lee

et al. 2022

Preprint

View full text Add to dashboard Cite

show abstract

“…This corroborates the value of introducing a sequence similarity-based feature in network inference strategies and highlights the importance of reducing the noise in a dataset before applying network inference methods. In addition, efforts have recently been made to identify the substrate recognition motifs for all kinases 43,44 , which will further improve our ability to reduce noise and match kinases to the correct substrates. Additional ways to reduce noise in the dataset could include filters to include phosphosites that are predicted to be functional 45 , and introducing very strict p-value and fold-change cut-offs for the identification of differentially abundant phosphosites.…”

Section: Discussionmentioning

confidence: 99%

Phosphoproteomics data-driven signalling network inference: does it work?

Sriraja

Werhli

Petsalaki

2022

Preprint

View full text Add to dashboard Cite

The advent in high throughput global phosphoproteome profiling has led to wide phosphosite coverage and therefore the need to predict kinase substrate associations from these datasets. However, for multiple substrates, the regulatory kinase is unknown due to biased and incomplete interactome databases. In this study we compare the performance of six pairwise measures to predict kinase substrate associations using a purely data driven approach on publicly available dynamic time resolved and perturbation phosphoproteome data using mass spectrometry profiling. First, we validated the performance of these measures using as a reference both a literature-based phosphosite-specific protein interaction network and a predicted kinase substrate (KS) interactions set. The overall performance in predicting kinase-substrate associations using pairwise measures across both database-derived and predicted interactomes was poor. To expand into the wider interactome space, the performance of these measures was evaluated against a network compiled from pairs of substrates regulated by the same kinase (substrate-substrate associations). Similar to the kinase substrate predictions, a purely statistical approach to predict substrate-substrate associations was also poor. However, the addition of a sequence similarity filter for substrate-substrate associations led to a boost in performance and to the inference of statistically significant substrate-substrate associations. Our findings imply that the use of a filter to reduce the search space, such as a sequence similarity filter, can be used prior to the application of network inference methods to reduce noise and boost the signal. We also find that the current gold standard for reference sets is not adequate for evaluation as it is limited and context-agnostic. Therefore, there is a need for additional evaluation methods that have increased coverage and take into consideration the context-specific nature of kinase substrate associations.

show abstract

“…Numerous mechanisms can underlie signaling specificity by protein kinases, including subcellular compartmentalization, scaffolding, signal dynamics, and direct kinase-substrate interactions 6 . One mechanism common to Ser/Thr protein kinases involves the recognition of sequence motifs surrounding sites of phosphorylation by the catalytic cleft 7 . However, since all MAPKs target a common Ser/Thr-Pro consensus sequence, catalytic site specificity is insufficient to mediate selectivity for a particular member of the family.…”

Section: Introductionmentioning

confidence: 99%

Linear motif specificity in signaling through p38α and ERK2 mitogen-activated protein kinases

Robles

Shi

Turk

2022

Preprint

Self Cite

View full text Add to dashboard Cite

Mitogen-activated protein kinase (MAPK) cascades are essential for eukaryotic cells to integrate and respond to a wide array of stimuli. Maintaining specificity in signaling through MAPK networks is key to coupling specific inputs to appropriate cellular responses. One way that MAPKs achieve specificity is through transient interactions with docking sites: short linear motifs found in MAPK substrates, regulators, and scaffolds. Docking sites bind to a conserved groove located in the catalytic domain of all MAPKs including the ERK and p38 subfamilies, but how specificity is achieved remains unresolved. To understand the basis of docking selectivity for these two subfamilies, we screened a library of thousands of human proteome-derived sequences for docking to ERK2 and p38α. We discovered a large number of sequences that bound specifically to only one MAPK or promiscuously to both, and that selective and non-selective interactors conformed to distinct sequence motifs. In particular, selective binding to p38α correlated with higher net charge in the docking site, and this phenomenon was driven by enrichment for Lys residues. A pair of acidic residues unique to the docking groove of p38α mediated selectivity for Lys-rich basic motifs. Finally, we validated a set of full-length proteins harboring docking sites selected as hits in our screens to be authentic MAPK interactors and identified ChREBP and TACC1 as cellular MAPK substrates. This study identifies distinguishing features that help define MAPK signaling networks and explains how specific docking motifs promote signaling integrity.

show abstract

A global atlas of substrate specificities for the human serine/threonine kinome

Cited by 20 publications

References 108 publications

High-throughput profiling of sequence recognition by tyrosine kinases and SH2 domains using bacterial peptide display

High-throughput profiling of sequence recognition by tyrosine kinases and SH2 domains using bacterial peptide display

Phosphoproteomics data-driven signalling network inference: does it work?

Linear motif specificity in signaling through p38α and ERK2 mitogen-activated protein kinases

Contact Info

Product

Resources

About