A PP2A-B55-Mediated Crosstalk between TORC1 and TORC2 Regulates the Differentiation Response in Fission Yeast

Martín, Ruth; Portantier, Marina; Chica, Nathalia; Nyquist-Andersen, Mari; Mata, Juan; López-Avilés, Sandra

doi:10.1016/j.cub.2016.11.037

Cited by 38 publications

(62 citation statements)

References 49 publications

(64 reference statements)

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“…We found that TORC1 controls SAGA through Ppk18 Gwlmediated inhibition of the PP2A B55 phosphatase. A very recent study proposed that a similar TORC1-activated signaling cascade inhibits sexual differentiation, through the de-phosphorylation of Gad8 AKT by PP2A B55 , thereby counteracting TORC2 activity [56]. Our work reveals that an additional substrate of the TORC1-PP2A B55 pathway contributes to control this process.…”

Section: Embo Reportssupporting

confidence: 59%

“…Interestingly, an S. pombe FOXO transcription factor, Fkh2, is also required for ste11 + induction and sexual differentiation upon nitrogen starvation [64] and is phosphorylated by Gad8 AKT in vitro [39]. Recently, a mutational analysis revealed that Gad8 AKT -dependent phosphorylation of Fkh2 is critical for sexual differentiation [56]. Our results show that Taf12 phosphorylation is induced early upon starvation, positively correlates with TORC2 activity, but not any other nutrient-sensing pathway, and negatively correlates with sexual differentiation.…”

Section: Embo Reportsmentioning

confidence: 99%

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TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

et al. 2017

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Gene expression regulation is essential for cells to adapt to changes in their environment. Co-activator complexes have well-established roles in transcriptional regulation, but less is known about how they sense and respond to signaling cues. We have previously shown that, in fission yeast, one such co-activator, the SAGA complex, controls gene expression and the switch from proliferation to differentiation in response to nutrient availability. Here, using a combination of genetic, biochemical, and proteomic approaches, we show that SAGA responds to nutrients through the differential phosphorylation of its Taf12 component, downstream of both the TORC1 and TORC2 pathways. Taf12 phosphorylation increases early upon starvation and is controlled by the opposing activities of the PP2A phosphatase, which is activated by TORC1, and the TORC2-activated Gad8 kinase. Mutational analyses suggest that Taf12 phosphorylation prevents cells from committing to differentiation until starvation reaches a critical level. Overall, our work reveals that SAGA is a direct target of nutrient-sensing pathways and has uncovered a mechanism by which TORC1 and TORC2 converge to control gene expression and cell fate decisions.

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Section: Embo Reportssupporting

confidence: 59%

Section: Embo Reportsmentioning

confidence: 99%

TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

et al. 2017

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“…These mutants are unable to cease cell growth, arrest with 1C DNA and sustain viability after nitrogen withdrawal (Sajiki et al, 2009;Sajiki, Tahara, Villar-Briones et al, 2018). TORC2 and Gad8, a downstream effector kinase of TORC2, were also reported to be required for cells to arrest with 1C DNA under −N and sexual differentiation (Ikeda, Morigasaki, Tatebe, Tamanoi, & Shiozaki, 2008;Martin et al, 2017;Matsuo, Kubo, Watanabe, & Yamamoto, 2003). Inhibition of PP2A Pab1 through the Ppk18/Cek1-Mug134 pathway may contribute to maintaining the state of phosphorylation of some substrates of these kinases which is important for proper entry into the G 0 phase.…”

Section: Discussionmentioning

confidence: 99%

The fission yeast Greatwall–Endosulfine pathway is required for proper quiescence/G₀ phase entry and maintenance

et al. 2019

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Cell proliferation and cellular quiescence/G0 phase must be regulated in response to intra‐/extracellular environments, and such regulation is achieved by the orchestration of protein kinases and protein phosphatases. Here, we investigated fission yeast potential orthologs (Cek1, Ppk18 and Ppk31) of the metazoan Greatwall kinase (Gwl), which inhibits type‐2A protein phosphatase with B55 subunit (PP2AB55) by phosphorylating and activating the PP2AB55 inhibitors, α‐endosulfine/ARPP‐19 (Ensa/ARPP‐19). Gwl and Ensa/ARPP‐19 regulate mitosis; however, we found Ppk18, Cek1 and Mug134/Igo1, the counterpart of Ensa/ARPP‐19, are not essential for normal mitosis but regulate nitrogen starvation (−N)‐induced proper G0 entry and maintenance. Genetic and biochemical analyses indicated that the conserved Gwl site (serine 64) was phosphorylated in the G0 phase in a Ppk18‐dependent manner, and the phosphorylated Mug134/Igo1 inhibited PP2AB55 in vitro. The alanine substitution of the serine 64 caused defects in G0 entry and maintenance as well as the mug134/igo1+ deletion. These results indicate that PP2AB55 activity must be regulated properly to establish the G0 phase. Consistently, simultaneous deletion of the B55 gene with mug134/igo1+ partially rescued the Mug134/Igo1 mutant phenotype. We suggest that in fission yeast, PP2AB55 regulation by the Ppk18‐Mug134/Igo1 pathway is required for G0 entry and establishment of robust viability during the G0 phase.

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“…Inactivation of TORC1 triggers the mating response [83,84], while deletion of TORC2 or its target Gad8 (the fission yeast orthologue of mammalian Akt) causes sterility [85]. Recently, it has been shown that the transition from cell growth to cell differentiation in response to nitrogen starvation, is regulated by PP2A/B55 phosphatase activity [38] through the dephosphorylation of Gad8 at Ser546 [37,82,86]. As indicated above, in low nitrogen, TORC1-Sck2 inactivation leads to the activation of the Greatwall-Endosulfine switch and therefore the inhibition of PP2A/B55, resulting in the accumulation of active Ser546 phosphorylated Gad8 and induction of the differentiation response.…”

Section: Pp2a/b55 Connects Torc1 and Torc2 And Provides A Switch Frommentioning

confidence: 99%

“…In Saccharomyces cerevisiae, TORC1 and protein kinase A (PKA) activities inhibit the Greatwall-Endosulfine switch, which is required for meiotic gene expression and survival in the G0 stationary phase [31][32][33][34]. By contrast, in fission yeast, the Greatwall-Endosulfine switch is negatively regulated by TORC1 [35], and it regulates cell size at division, entry into quiescence [36], and the sexual differentiation response [37,38].…”

Section: Introductionmentioning

confidence: 99%

Greatwall-Endosulfine: A Molecular Switch that Regulates PP2A/B55 Protein Phosphatase Activity in Dividing and Quiescent Cells

García-Blanco

Vázquez-Bolado

Moreno

2019

IJMS

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During the cell cycle, hundreds of proteins become phosphorylated and dephosphorylated, indicating that protein kinases and protein phosphatases play a central role in its regulation. It has been widely recognized that oscillation in cyclin-dependent kinase (CDK) activity promotes DNA replication, during S-phase, and chromosome segregation, during mitosis. Each CDK substrate phosphorylation status is defined by the balance between CDKs and CDK-counteracting phosphatases. In fission yeast and animal cells, PP2A/B55 is the main protein phosphatase that counteracts CDK activity. PP2A/B55 plays a key role in mitotic entry and mitotic exit, and it is regulated by the Greatwall-Endosulfine (ENSA) molecular switch that inactivates PP2A/B55 at the onset of mitosis, allowing maximal CDK activity at metaphase. The Greatwall-ENSA-PP2A/B55 pathway is highly conserved from yeast to animal cells. In yeasts, Greatwall is negatively regulated by nutrients through TORC1 and S6 kinase, and couples cell growth, regulated by TORC1, to cell cycle progression, driven by CDK activity. In animal cells, Greatwall is phosphorylated and activated by Cdk1 at G2/M, generating a bistable molecular switch that results in full activation of Cdk1/CyclinB. Here we review the current knowledge of the Greatwall-ENSA-PP2A/B55 pathway and discuss its role in cell cycle progression and as an integrator of nutritional cues.

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A PP2A-B55-Mediated Crosstalk between TORC1 and TORC2 Regulates the Differentiation Response in Fission Yeast

Cited by 38 publications

References 49 publications

TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

The fission yeast Greatwall–Endosulfine pathway is required for proper quiescence/G₀ phase entry and maintenance

Greatwall-Endosulfine: A Molecular Switch that Regulates PP2A/B55 Protein Phosphatase Activity in Dividing and Quiescent Cells

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A PP2A-B55-Mediated Crosstalk between TORC1 and TORC2 Regulates the Differentiation Response in Fission Yeast

Cited by 38 publications

References 49 publications

TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

TORC1 and TORC2 converge to regulate the SAGA co‐activator in response to nutrient availability

The fission yeast Greatwall–Endosulfine pathway is required for proper quiescence/G0 phase entry and maintenance

Greatwall-Endosulfine: A Molecular Switch that Regulates PP2A/B55 Protein Phosphatase Activity in Dividing and Quiescent Cells

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The fission yeast Greatwall–Endosulfine pathway is required for proper quiescence/G₀ phase entry and maintenance