2015
DOI: 10.1073/pnas.1423344112
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Empirical inference of circuitry and plasticity in a kinase signaling network

Abstract: Our understanding of physiology and disease is hampered by the difficulty of measuring the circuitry and plasticity of signaling networks that regulate cell biology, and how these relate to phenotypes. Here, using mass spectrometry-based phosphoproteomics, we systematically characterized the topology of a network comprising the PI3K/Akt/mTOR and MEK/ERK signaling axes and confirmed its biological relevance by assessing its dynamics upon EGF and IGF1 stimulation. Measuring the activity of this network in models… Show more

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Cited by 73 publications
(116 citation statements)
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“…18). Phosphopeptide abundance—directly relating to the amount of substrate phosphorylation—was determined by a label-free quantitative analysis1920 (Supplementary Dataset 1). Substrate phosphorylation was assessed when PKGIα was activated by the Cys42 disulfide bond or via the classical pathway with cGMP, and compared with phosphorylation when PKGIα was in its basal ‘unactivated' state (control; Fig.…”
Section: Resultsmentioning
confidence: 99%
See 1 more Smart Citation
“…18). Phosphopeptide abundance—directly relating to the amount of substrate phosphorylation—was determined by a label-free quantitative analysis1920 (Supplementary Dataset 1). Substrate phosphorylation was assessed when PKGIα was activated by the Cys42 disulfide bond or via the classical pathway with cGMP, and compared with phosphorylation when PKGIα was in its basal ‘unactivated' state (control; Fig.…”
Section: Resultsmentioning
confidence: 99%
“…The abundance of phosphopeptides in each of the kinase reaction mixtures described above was determined by a label-free quantitative phosphoproteomic analysis1920. LC–MS/MS analysis was performed on an Ultimate 3000, nLC system (ThermoFisher) connected to an LTQ Orbitrap XL instrument to.…”
Section: Methodsmentioning
confidence: 99%
“…Samples were processed as described60, with the following modifications. Primary MEFs were lysed 48 or 96 h after 4-OHT treatment in 1 ml of urea buffer per 15 cm tissue culture dish.…”
Section: Methodsmentioning
confidence: 99%
“…Importantly, single shot nanoLC- [17,22,23], the current pTyrphosphoproteomics workflow requires protein input of typically 10-20 mg per sample, corresponding to about 100-200 mg tissue wet weight [14]. In this study, we downscaled protein input to the clinically feasible needle biopsy-level of 1 mg protein per sample and…”
Section: Accepted Manuscriptmentioning
confidence: 99%