Abstract
SHP2 was recently found to down-regulate PI3K activation by dephosphorylating Gab1 but the mechanisms explaining the positive role of the Gab1/SHP2 pathway in EGF-induced Ras activation remain ill defined. Substrate trapping experiments now suggest that SHP2 dephosphorylates other Gab1 phosphotyrosines located within a central region displaying four YXXP motifs. Because these sites are potential docking motifs for Ras-GAP, we tested whether SHP2 dephosphorylates them to facilitate Ras activation. We observed that a Gab1 construct preventing SHP2 recruitment promoted membrane relocation of RasGAP. Moreover, a RasGAP-inactive mutant restored the activation of Ras in cells transfected with SHP2-inactivating Gab1 mutant or in SHP2-deficient fibroblasts, supporting the hypothesis that RasGAP is a downstream target of SHP2. To determine whether Gab1 is a RasGAP-binding partner, a Gab1 mutant deleted of four YXXP motifs was produced. The deletion suppressed RasGAP redistribution and restored the defective Ras activation caused by SHP2-inactivating mutations. Moreover, Gab1 was found to interact with RasGAP SH2 domains, only under conditions where SHP2 is not activated. To identify Ras-GAP-binding sites, Tyr to Phe mutants of Gab1 YXXP motifs were produced. Gab1 constructs mutated on Tyr(317) were severely affected in RasGAP binding and were the most active in compensating for Ras-defective activation and blocking RasGAP redistribution induced by SHP2 inactivation. We have thus localized on Gab1 a Ras-negative regulatory tyrosine phosphorylation site involved in RasGAP binding and showed that an important SHP2 function is to down-regulate its phosphorylation to disengage RasGAP and sustain Ras activation.
Highlights
The GTPase Ras is a crucial signaling relay of receptor tyrosine kinases, and the mechanisms controlling its activation by growth factors appear well understood
The catalytic activity of SHP2 is important for Ras/Erk activation induced by epidermal growth factor (EGF), insulin, or hepatocyte growth factor, which implies that SHP2 does not growth factor; PI3K, phosphoinositide 3-kinase; Ras-binding domain (RBD), Ras-GTP binding domain; SH, Src homology; SHP2-C/S, SHP2 catalytically inactive mutant; WT, wild-type; Erk1/2, extracellular signal-regulated kinases 1 and 2; MEF, mouse embryo fibroblast; C/S, C459S mutant; 2RQ, R789Q/R903Q double mutant
It was only known that SHP2 can dephosphorylate Gab1 PI3K-binding sites [18], and, unlikely, it was necessary to exclude that dephosphorylation of Gab1 YXXM motifs could be somehow positive for Ras activation
Summary
The GTPase Ras is a crucial signaling relay of receptor tyrosine kinases, and the mechanisms controlling its activation by growth factors appear well understood. Using substrate trapping and site-directed mutagenesis, we have obtained evidence that Gab1 YXXP motifs can recruit RasGAP and that an essential function of SHP2 is to down-regulate this interaction, allowing an efficient activation of Ras in response to EGF.
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