Activation of p70s6k is associated with phosphorylation of four clustered sites displaying Ser/Thr-Pro motifs.

Ferrari, Stefano; Bannwarth, Willi; Morley, Simon; Totty, Nicholas F.; Thomas, George

doi:10.1073/pnas.89.15.7282

Cited by 158 publications

(133 citation statements)

References 52 publications

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“…We have investigated the contribution of these pathways to the di erentiation process by the use of chemical inhibitors. P70S6K was inhibited with the immunosuppressant rapamycin (Ferrari et al, 1992). To inhibit the a and b isoforms of p38-MAPK we used the pyridinyl imidazole compound PD169316 (PD*) (Kummer et al, 1997).…”

Section: Insulin (In the Presence Of Pd) Produces C2ras Myotubes In Amentioning

confidence: 99%

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

et al. 2002

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v-H-ras transformed C2C12 (C2Ras) myoblasts, overexpressing p21-Ras protein in the Ras-GTP active form, showed a di erentiation-defective phenotype when cultured in low serum as compared with C2C12 myoblasts. Accordingly, the purpose of the present study was to delineate the signaling pathways that restore C2Ras myoblasts di erentiation. Inhibition of p42/p44-MAPK with the chemical inhibitor PD98059, and activation of AKT/P70S6K and p38-MAPK with insulin, produced growth arrest (precluding the expression of PCNA, cyclin-D1 and retinoblastoma at the hyperphosphorylated state and inducing the expression of the cell cycle inhibitor p21 Cip ) and myogenesis (multinucleated myotubes formation and induction of creatine kinase, caveolin-3 and a-actin). Both events were accompanied by down-regulation of AP-1 and up-regulation of NF-kB transcriptional activities. Furthermore, inhibition of NFkB transcriptional activity by the use of the proteasome inhibitor MG132 totally precluded di erentiation by insulin+PD98059, demonstrating a direct role for NFkB on C2Ras myogenesis. C2Ras myoblasts failed to restore di erentiation when rapamycin or PD169316 were added in the presence of insulin+PD98059, indicating that the activation of both P70S6K and p38-MAPK was necessary to reach a fully di erentiated phenotype. Finally, transient transfection of a constitutively active Myr-EGFP-AKT-HA construct (in the presence of PD98059) restored C2Ras myogenesis by its ability to activate P70S6K and p38-MAPK. A crosstalk between P70S6K and p38-MAPK was observed under rapamycin treatment in both insulin or active AKT induced myogenesis. Our results are delineating an AKT/ P70S6K/p38-MAPK pathway involved in skeletal muscle di erentiation.

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Section: Insulin (In the Presence Of Pd) Produces C2ras Myotubes In Amentioning

confidence: 99%

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

et al. 2002

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“…In parallel it has been demonstrated that the immunosuppressant rapamycin, a bacterial macrolide, negates mitogen-induced activation of p70 s6k by preventing the acute phosphorylation of a specific subset of sites, including T 229 , T 389 , S 404 , and S 411 (54). These sites were found to be flanked by large aromatic residues, with the exception of S 411 , which exhibits an S/TP motif, as do the remaining three unaffected phosphorylation sites (18,54). Of the rapamycin-sensitive sites, the principal site of rapamycin-induced dephosphorylation leading to p70 s6k inactivation was identified as T 389 , which resides in the linker region, coupling the catalytic and autoinhibitory domains (54).…”

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confidence: 99%

The Insulin-Induced Signalling Pathway Leading to S6 and Initiation Factor 4E Binding Protein 1 Phosphorylation Bifurcates at a Rapamycin-Sensitive Point Immediately Upstream of p70^s6k

Manteuffel

Dennis

Pullen

et al. 1997

Molecular and Cellular Biology

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Employing specific inhibitors and docking-site mutants of growth factor receptors, recent studies have indicated that the insulin-induced increase in 40S ribosomal protein S6 and initiation factor 4E binding protein 1 (4E-BP1) phosphorylation is mediated by the mTOR/FRAP-p70 s6k signal transduction pathway. However, it has not been resolved whether the phosphorylation of both proteins is mediated by p70 s6k or whether they reside on parallel pathways which bifurcate upstream of p70 s6k . Here we have used either rapamycin-resistant, kinase-dead, or wild-type p70 s6k variants to distinguish between these possibilities. The rapamycin-resistant p70 s6k , which has high constitutive activity, was able to signal to S6 in the absence of insulin and to prevent the rapamycin-induced block of S6 phosphorylation. This same construct did not increase the basal state of 4E-BP1 phosphorylation or protect it from the rapamycin-induced block in phosphorylation. Unexpectedly, the rapamycin-resistant p70 s6k inhibited insulin-induced 4E-BP1 phosphorylation in a dose-dependent manner. This effect was mimicked by the kinase-dead and wild-type p70 s6k constructs, which also blocked insulininduced dissociation of 4E-BP1 from initiation factor 4E. Both the kinase-dead and wild-type constructs also blocked reporter p70 s6k activation, although only the kinase-dead p70 s6k had a dominant-interfering effect on S6 phosphorylation. Analysis of phosphopeptides from reporter 4E-BP1 and p70 s6k revealed that the kinasedead p70 s6k affected the same subset of sites as rapamycin in both proteins. The results demonstrate, for the first time, that activated p70 s6k mediates increased S6 phosphorylation in vivo. Furthermore, they show that increased 4E-BP1 phosphorylation is controlled by a parallel signalling pathway that bifurcates immediately upstream of p70 s6k , with the two pathways sharing a common rapamycin-sensitive activator.In insulin-responsive cells, hormonal stimulation provokes the coordinate activation of a complex network of signalling pathways which are involved in the regulation of specific metabolic processes (71). Critical among these affected metabolic processes is the activation and maintenance of high rates of protein synthesis, leading to both global and selective changes in the pattern of translation (14,23,56). Recent studies have suggested that in insulin-sensitive tissues, such as liver, heart, skeletal muscle, and adipose tissue, the increase in protein synthesis is triggered by ligand-induced activation of the receptor and propagated intracellularly through the phosphorylation of the insulin receptor substrate IRS-1 (66). IRS-1 is thought to mediate the insulin signal by inducing the activation of distinct kinases which then target specific components of the translational apparatus (45). In several cases, there is considerable knowledge concerning the functional roles of specific translational components in protein synthesis and of the effect of phosphorylation on their individual activities (48, 65). Much less is k...

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“…Furthermore, incubation of p70 S6K with synthetic peptides derived from this homologous region substantially hinders its activation (68, 69) demonstrating that this module, in the context of the full-length p70 S6K polypeptide, may serve an autoinhibitory function. Stimulation of cells in culture with growth factors initiates signals that lead to the hierarchical activation of p70 S6K, commencing with the (Ser/Thr)Pro-specific phosphorylation of a cluster of 4 -6 residues with the carboxyl terminus of the kinase (19). This battery of phosphorylations promotes a conformational change that relieves autoinhibition imposed by the carboxyl terminus and, in addition, exposes additional phosphorylation sites initially buried within interior of p70 S6K.…”

Section: Transcriptional Scenarios Involved In Regulation Of P70 S6kmentioning

confidence: 99%

“…Two key observations support this premise. First, the primary amino acid sequence surrounding the cluster of p70 S6K carboxyl-terminal phosphorylation sites exhibits strong homology to the region within its substrate, S6, that it phosphorylates (19,68); hence, the designation "pseudosubstrate" domain. Furthermore, incubation of p70 S6K with synthetic peptides derived from this homologous region substantially hinders its activation (68, 69) demonstrating that this module, in the context of the full-length p70 S6K polypeptide, may serve an autoinhibitory function.…”

Section: Transcriptional Scenarios Involved In Regulation Of P70 S6kmentioning

confidence: 99%

“…1A). These phosphorylations occur in a hierarchical manner commencing with phosphorylation of a cluster of at least four carboxyl-terminal sites localized within the presumptive autoinhibitory pseudosubstrate domain (19). These phosphorylation events have been suggested to transform the conformation of the protein so as to disrupt a putative interaction between the autoinhibitory region and the substrate recognition pocket.…”

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confidence: 99%

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The Activated Glucocorticoid Receptor Modulates Presumptive Autoregulation of Ribosomal Protein S6 Protein Kinase, p70 S6K

Shah

Iñiguez‐Lluhí

Romanelli

et al. 2002

Journal of Biological Chemistry

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Protein metabolism in eukaryotic organisms is defined by a synthesis-degradation equilibrium that is subject to regulation by hormonal and nutritional signals. In mammalian tissues such as skeletal muscle, glucocorticoid hormones specify a catabolic response that influences both protein synthetic and protein degradative pathways. With regard to the former, glucocorticoids attenuate mRNA translation at two levels: translational efficiency, i.e. translation initiation, and translational capacity, i.e. ribosome biogenesis. Glucocorticoids may impair translational capacity through the ribosomal S6 protein kinase (p70 S6K), a recognized glucocorticoid target and an effector of ribosomal protein synthesis. We demonstrate here that the reduction in growth factor-activated p70 S6K activity by glucocorticoids depends upon a functional glucocorticoid receptor (GR) and that the GR is both necessary and sufficient to render p70 S6K subject to glucocorticoid regulation. Furthermore, the DNA binding and transcriptional activation but not repression properties of the GR are indispensable for p70 S6K regulation. Finally, a mutational analysis of the p70 S6K carboxyl terminus indicates that this region confers glucocorticoid sensitivity, and thus glucocorticoids may facilitate autoinhibition of the enzyme ultimately reducing the efficiency with which T389 is phosphorylated.

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Activation of p70s6k is associated with phosphorylation of four clustered sites displaying Ser/Thr-Pro motifs.

Cited by 158 publications

References 52 publications

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

The Insulin-Induced Signalling Pathway Leading to S6 and Initiation Factor 4E Binding Protein 1 Phosphorylation Bifurcates at a Rapamycin-Sensitive Point Immediately Upstream of p70^s6k

The Activated Glucocorticoid Receptor Modulates Presumptive Autoregulation of Ribosomal Protein S6 Protein Kinase, p70 S6K

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Activation of p70s6k is associated with phosphorylation of four clustered sites displaying Ser/Thr-Pro motifs.

Cited by 158 publications

References 52 publications

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

Insulin restores differentiation of Ras-transformed C2C12 myoblasts by inducing NF-κB through an AKT/P70S6K/p38-MAPK pathway

The Insulin-Induced Signalling Pathway Leading to S6 and Initiation Factor 4E Binding Protein 1 Phosphorylation Bifurcates at a Rapamycin-Sensitive Point Immediately Upstream of p70s6k

The Activated Glucocorticoid Receptor Modulates Presumptive Autoregulation of Ribosomal Protein S6 Protein Kinase, p70 S6K

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The Insulin-Induced Signalling Pathway Leading to S6 and Initiation Factor 4E Binding Protein 1 Phosphorylation Bifurcates at a Rapamycin-Sensitive Point Immediately Upstream of p70^s6k