Literature DB >> 31585087

Oncogenic Mutations Rewire Signaling Pathways by Switching Protein Recruitment to Phosphotyrosine Sites.

Alicia Lundby1, Giulia Franciosa2, Kristina B Emdal2, Jan C Refsgaard2, Sebastian P Gnosa3, Dorte B Bekker-Jensen2, Anna Secher4, Svetlana R Maurya5, Indranil Paul2, Blanca L Mendez2, Christian D Kelstrup2, Chiara Francavilla2, Marie Kveiborg3, Guillermo Montoya2, Lars J Jensen2, Jesper V Olsen6.   

Abstract

Tyrosine phosphorylation regulates multi-layered signaling networks with broad implications in (patho)physiology, but high-throughput methods for functional annotation of phosphotyrosine sites are lacking. To decipher phosphotyrosine signaling directly in tissue samples, we developed a mass-spectrometry-based interaction proteomics approach. We measured the in vivo EGF-dependent signaling network in lung tissue quantifying >1,000 phosphotyrosine sites. To assign function to all EGF-regulated sites, we determined their recruited protein signaling complexes in lung tissue by interaction proteomics. We demonstrated how mutations near tyrosine residues introduce molecular switches that rewire cancer signaling networks, and we revealed oncogenic properties of such a lung cancer EGFR mutant. To demonstrate the scalability of the approach, we performed >1,000 phosphopeptide pulldowns and analyzed them by rapid mass spectrometric analysis, revealing tissue-specific differences in interactors. Our approach is a general strategy for functional annotation of phosphorylation sites in tissues, enabling in-depth mechanistic insights into oncogenic rewiring of signaling networks.
Copyright © 2019 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  EGFR; SH2; cancer signaling; interaction proteomics; mass spectrometry; peptide pulldown; phosphopeptides; phosphoproteomics; phosphotyrosine; zebrafish

Mesh:

Substances:

Year:  2019        PMID: 31585087     DOI: 10.1016/j.cell.2019.09.008

Source DB:  PubMed          Journal:  Cell        ISSN: 0092-8674            Impact factor:   41.582


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