Literature DB >> 24275748

Characterization of early autophagy signaling by quantitative phosphoproteomics.

Kristoffer Tg Rigbolt1, Mostafa Zarei1, Adrian Sprenger2, Andrea C Becker1, Britta Diedrich1, Xun Huang3, Sven Eiselein4, Anders R Kristensen5, Christine Gretzmeier1, Jens S Andersen6, Zhike Zi3, Jörn Dengjel7.   

Abstract

Under conditions of nutrient shortage autophagy is the primary cellular mechanism ensuring availability of substrates for continuous biosynthesis. Subjecting cells to starvation or rapamycin efficiently induces autophagy by inhibiting the MTOR signaling pathway triggering increased autophagic flux. To elucidate the regulation of early signaling events upon autophagy induction, we applied quantitative phosphoproteomics characterizing the temporal phosphorylation dynamics after starvation and rapamycin treatment. We obtained a comprehensive atlas of phosphorylation kinetics within the first 30 min upon induction of autophagy with both treatments affecting widely different cellular processes. The identification of dynamic phosphorylation already after 2 min demonstrates that the earliest events in autophagy signaling occur rapidly after induction. The data was subjected to extensive bioinformatics analysis revealing regulated phosphorylation sites on proteins involved in a wide range of cellular processes and an impact of the treatments on the kinome. To approach the potential function of the identified phosphorylation sites we performed a screen for MAP1LC3-interacting proteins and identified a group of binding partners exhibiting dynamic phosphorylation patterns. The data presented here provide a valuable resource on phosphorylation events underlying early autophagy induction.

Entities:  

Keywords:  autophagy; bioinformatics; mass spectrometry; phosphoproteomics; phosphorylation; proteomics; signal transduction

Mesh:

Substances:

Year:  2013        PMID: 24275748      PMCID: PMC5396084          DOI: 10.4161/auto.26864

Source DB:  PubMed          Journal:  Autophagy        ISSN: 1554-8627            Impact factor:   16.016


  76 in total

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4.  Comparison of ERLIC-TiO2, HILIC-TiO2, and SCX-TiO2 for global phosphoproteomics approaches.

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4.  Phosphoproteome-based kinase activity profiling reveals the critical role of MAP2K2 and PLK1 in neuronal autophagy.

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5.  Studying Autophagy Using a TMT-Based Quantitative Proteomics Approach.

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10.  Inducing autophagy: a comparative phosphoproteomic study of the cellular response to ammonia and rapamycin.

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