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Interaction with phospho-eIF4E commits S6 Kinase 1 for mTORC2 and PHLPP1 mediated activation

biorxiv. 2020; 
Sheikh Tahir Majeed, Asiya Batool, Rabiya Majeed, Nadiem Nazir Bhat, Khurshid Iqbal Andrabi
Products/Services Used Details Operation
Recombinant Proteins PVDF membrane (GE Healthcare/Millipore), Rapamycin (Sigma Aldrich) and Mnk1 inhibitor (Merck USA), Protein G-Agarose beads (Genscript), Torin (Tocris), Glutathione agarose beads (Thermo-scientific). Polyetheleneimine reagent (Polysciences, Inc.), Radioactive ATP (BRIT, Hyderabad-India). Antibodies against p-S6K1(T389/T412), p-eIF4E(S209), mTOR, Raptor, ULK1, S6, Flag-tag were bought from Cell Signaling Technologies (Beverly MA); HA-tag, myc-tag, tubulin, GST and GAPDH (Sigma-Aldrich); 4E-BP1 and eIF4E (Abcam); β-actin (Thermo Scientific), rabbit and mouse secondary antibodies conjugated to IR Dye 800CW (LI-COR Biotechnology, Lincoln, Nebraska); S6K1 (GenScript) Get A Quote

摘要

Eukaryotic initiation factor (eIF4E) phosphorylation is a recognized attribute for enhanced cell growth and proliferation. Our recent data that identifies eIF4E as mTORC1 substrate with ability to influence rapamycin response highlights its prospect as a mediator of mTORC1 signaling. Here, we present evidence that eIF4E phosphorylated at S209 interacts with TOS motif of S6 Kinase1 (S6K1). We show that this interaction is sufficient to overcome rapamycin sensitivity and mTORC1 dependence of S6K1. We present data to demonstrate that eIF4E-S6K1 interaction serves to relieve S6K1 of its carboxy terminal auto inhibition, otherwise rate limiting for its activation. We go on to identify a highly conserved sequence seg... More

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