Multi-signal regulation of the GSK-3β homolog Rim11 controls meiosis entry in budding yeast

Author:

Kociemba Johanna,Jørgensen Andreas Christ Sølvsten,Tadić Nika,Harris AnthonyORCID,Sideri Theodora,Chan Wei Yee,Ibrahim Fairouz,Ünal Elçin,Skehel Mark,Shahrezaei VahidORCID,Argüello-Miranda OrlandoORCID,van Werven Folkert JacobusORCID

Abstract

AbstractStarvation in diploid budding yeast cells triggers a cell-fate program culminating in meiosis and spore formation. Transcriptional activation of early meiotic genes (EMGs) hinges on the master regulator Ime1, its DNA-binding partner Ume6, and GSK-3β kinase Rim11. Phosphorylation of Ume6 by Rim11 is required for EMG activation. We report here that Rim11 functions as the central signal integrator for controlling Ume6 phosphorylation and EMG transcription. In nutrient-rich conditions, PKA suppresses Rim11 levels, while TORC1 retains Rim11 in the cytoplasm. Inhibition of PKA and TORC1 induces Rim11 expression and nuclear localization. Remarkably, nuclear Rim11 is required, but not sufficient, for Rim11-dependent Ume6 phosphorylation. In addition, Ime1 is an anchor protein enabling Ume6 phosphorylation by Rim11. Subsequently, Ume6-Ime1 coactivator complexes form and induce EMG transcription. Our results demonstrate how various signaling inputs (PKA/TORC1/Ime1) converge through Rim11 to regulate EMG expression and meiosis initiation. We posit that the signaling-regulatory network elucidated here generates robustness in cell-fate control.

Funder

Wellcome Trust

UKRI | MRC | Medical Research Foundation

Cancer Research UK

HHS | NIH | National Institute of General Medical Sciences

Publisher

Springer Science and Business Media LLC

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