Positive and negative feedback loops affect the transcription of <i>IME1</i>, a positive regulator of meiosis in <i>Saccharomyces cerevisiae</i>

Shefer‐Vaida, Michal; Sherman, Amir; Ashkenazi, Tamar; Robzyk, Kenneth; Kassir, Yona

doi:10.1002/dvg.1020160302

Cited by 27 publications

(41 citation statements)

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“…Expression of Ime2p leads to the eventual repression of IME1 transcription during late stages of meiosis (Shefer-Vaida et al, 1995;Smith and Mitchell, 1989). More directly, Ime2p kinase may phosphorylate Ime1p and target it for degradation (Guttmann-Raviv et al, 2002).…”

Section: Ime2 Repression Of Ime1mentioning

confidence: 99%

Signal pathway integration in the switch from the mitotic cell cycle to meiosis in yeast

Honigberg

Purnapatre

2003

Journal of Cell Science

131

136

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Diploid yeast, like most eukaryotes, can undergo meiotic differentiation to form haploid gametes. Meiotic differentiation and cell growth (proliferation)are mutually exclusive programs, and in yeast the switch between growth and meiosis is controlled by nutritional signals. The signaling pathways that mediate nutritional controls on meiotic initiation fall into three broad classes: those that respond to nutrient starvation, those that respond to non-fermentable carbon sources, and those that respond to glucose. At the onset of meiosis, nutritional signaling pathways converge on transcriptional regulation of two genes: IME1, which encodes a transcription factor;and IME2, which encodes a protein kinase. Transcription of IME1 and IME2 trigger initiation of meiosis, and the expression of these two genes is linked with one other, with expression of later meiotic genes and with early meiotic events such as DNA replication. In addition, the signaling pathways that control IME1 and IME2expression are themselves integrated through a variety of mechanisms. Thus the signal network that controls the switch from growth to meiotic differentiation provides a signaling code that translates different combinations of extracellular signals into appropriate cellular responses.

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Section: Ime2 Repression Of Ime1mentioning

confidence: 99%

Signal pathway integration in the switch from the mitotic cell cycle to meiosis in yeast

Honigberg

Purnapatre

2003

Journal of Cell Science

131

136

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“…Under meiotic conditions, i.e., nitrogen depletion and the presence of a nonfermentable carbon source such as acetate, transcription of IME1 is induced transiently in MATa/ MAT␣ diploids (22). It is not known whether this transient transcription reflects transient availability of the Ime1 protein.In addition, the IME1 promoter is subject to positive autoregulation (40,43,44), as well as negative-feedback regulation by both Ime1 and Ime2 (43,48,49).Another important regulator of meiosis and sporulation is the serine/threonine protein kinase Ime2 (12,24,34,48,49). Diploid cells with deletions of IME2 show a 5-to 12-h delay in the transcription of early meiosis-specific genes, a reduction in their level of expression, and extremely low RNA levels of middle and late genes (34,49).…”

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confidence: 99%

Ime2, a Meiosis-Specific Kinase in Yeast, Is Required for Destabilization of Its Transcriptional Activator, Ime1

Guttmann‐Raviv

Martin

Kassir

2002

Molecular and Cellular Biology

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In the budding yeast Saccharomyces cerevisiae, entry into meiosis and its successful completion depend on two positive regulators, Ime1 and Ime2. Ime1 is a transcriptional activator that is required for transcription of IME2, a serine/threonine protein kinase. We show that in vivo Ime2 associates with Ime1, that in vitro Ime2 phosphorylates Ime1, and that in living cells the stability of Ime1 depends on Ime2. Diploid cells with IME2 deleted show an increase in the level of Ime1, whereas haploid cells overexpressing IME2 show a decrease in the stability of Ime1. Furthermore, the level of Ime1 depends on the kinase activity of Ime2. Using a mutation in one of the ATPase subunits of the proteasome, RPT2, we demonstrate that Ime1, amino acids 270 to 360, is degraded by the 26S proteasome. We also show that Ime2 itself is an extremely unstable protein whose expression in vegetative cultures is toxic. We propose that a negative-feedback loop ensures that the activity of Ime1 will be restricted to a narrow window.Successful progression and completion of the mitotic cell cycle depends on transcriptional and proteolytic regulation. These two processes determine the availability of cyclins and cyclin-dependent kinase (CDK) inhibitors that govern the sequential activation of CDKs (18,28,31,35). Initiation and progression through the meiotic cycle should also be subjected to transcriptional and proteolytic regulation. Indeed, in budding yeast a transcriptional cascade governs initiation and progression through the meiotic cell cycle (4). Yet there is no direct evidence concerning proteolysis of either positive or negative meiotic regulators. This report focuses on the regulated degradation of one of the two positive regulators of meiosis in Saccharomyces cerevisiae, Ime1, by the other, Ime2.IME1 encodes a transcriptional activator (30, 47) that is necessary for the transcription of meiosis-specific genes (48). Ime1 is tethered to promoters of early meiosis-specific genes, such as IME2, by a specific DNA-binding protein, Ume6 (39). Diploid cells with deletions of IME1 arrest at G 1 prior to the initiation of premeiotic DNA replication (22). The transcription of IME1 is regulated by nutrients. In vegetative cultures with glucose as the sole carbon source, IME1 is silent, but in the presence of acetate, low levels of IME1 mRNA are observed (22). Under meiotic conditions, i.e., nitrogen depletion and the presence of a nonfermentable carbon source such as acetate, transcription of IME1 is induced transiently in MATa/ MAT␣ diploids (22). It is not known whether this transient transcription reflects transient availability of the Ime1 protein.In addition, the IME1 promoter is subject to positive autoregulation (40,43,44), as well as negative-feedback regulation by both Ime1 and Ime2 (43,48,49).Another important regulator of meiosis and sporulation is the serine/threonine protein kinase Ime2 (12,24,34,48,49). Diploid cells with deletions of IME2 show a 5-to 12-h delay in the transcription of early meiosis-specific genes, a reduction...

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“…The Ime2 protein abundance in rich medium is 538 molecules per cell (Lu et al, 2006), and this number is assumed as the basal level of each proteins in our model (10-11nM). As the maximum Ime1 protein expression level is around relative levels of 6 and 7 (ȕ-gal units: 60 and 70) in (SheferǦVaida et al, 1995), the maximum protein level is then approximately 100nM. Considering the maximum Ime1 protein expression relative level of 6 (SheferǦVaida et al, 1995), and as the experiments revealed that Rpd3/Sin3 is at its maximum activity at early stage (Pnueli et al, 2004;Rubinstein et al, 2007), initial condition for Rpd3/Sin3 is decided as 60nM (6 times from the basal level).…”

Section: Typical Meiosis Initiation Conditions Include Low Basal Levementioning

confidence: 95%

“…(Ray et al, 2013) (Rubinstein et al, 2007)). Further, the model is not validated with the available experimental data of the temporal behaviour of the Ime1 and Ime2 protein expressions (Nachman et al, 2007;SheferǦVaida et al, 1995).…”

Section: Introductionmentioning

confidence: 95%

A nutrient dependant switch explains mutually exclusive existence of meiosis and mitosis initiation in budding yeast

Wannige

Kulasiri

Samarasinghe

2014

Journal of Theoretical Biology

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Nutrients from living environment are vital for the survival and growth of any organism.Budding yeast diploid cells decide to grow by mitosis type cell division or decide to create unique, stress resistant spores by meiosis type cell division depending on the available nutrient conditions. To gain a molecular systems level understanding of the nutrient dependant switching between meiosis and mitosis initiation in diploid cells of budding yeast, we develop a theoretical model based on ordinary differential equations (ODEs) including the mitosis initiator and its relations to budding yeast meiosis initiation network. Our model accurately and qualitatively predicts the experimentally revealed temporal variations of related proteins under different nutrient conditions as well as the diverse mutant studies related to meiosis and mitosis initiation. Using this model, we show how the meiosis and mitosis initiators form an all-or-none type bistable switch in response to available nutrient level (mainly nitrogen). The transitions to and from meiosis or mitosis initiation states occur via saddle node bifurcation. This bidirectional switch helps the optimal usage of available nutrients and explains the mutually exclusive existence of meiosis and mitosis pathways.Key words: Bistable switching; Negative-feedback; Bifurcation; Saccharomyces cerevisiae Authors' contributions: The first and second authors developed the conceptual and mathematical models; the first author did all the computational work; the third author contributed to the data analysis, parameter estimation and clarifications related to the cell cycle; the first and second author wrote the paper with third author's assistance.

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Positive and negative feedback loops affect the transcription of IME1, a positive regulator of meiosis in Saccharomyces cerevisiae

Cited by 27 publications

References 28 publications

Signal pathway integration in the switch from the mitotic cell cycle to meiosis in yeast

Signal pathway integration in the switch from the mitotic cell cycle to meiosis in yeast

Ime2, a Meiosis-Specific Kinase in Yeast, Is Required for Destabilization of Its Transcriptional Activator, Ime1

A nutrient dependant switch explains mutually exclusive existence of meiosis and mitosis initiation in budding yeast

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