Whi5 Regulation by Site Specific CDK-Phosphorylation in Saccharomyces cerevisiae

Wagner, Michelle V.; Smolka, Marcus B.; Bruin, Rob A. M. de; Zhou, Huilin; Wittenberg, Curt; Dowdy, Steven F.

doi:10.1371/journal.pone.0004300

Cited by 70 publications

(111 citation statements)

References 45 publications

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“…Using these conditions, we monitored Whi5 gel mobility (Figure 6A), which reflects CDK phosphorylation [9, 10, 12]. V5-tagged Whi5 was resolved into three species: one in G1 arrested cells, plus two higher forms that appeared after release (Figure 6Ai–ii).…”

Section: Resultsmentioning

confidence: 99%

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

et al. 2015

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Summary Background Eukaryotic cell division is driven by cyclin-dependent kinases (CDKs). Distinct cyclin-CDK complexes are specialized to drive different cell cycle events, though the molecular foundations for these specializations are only partly understood. In budding yeast, the decision to begin a new cell cycle is regulated by three G1 cyclins (Cln1–Cln3). Recent studies revealed that some CDK substrates contain a novel docking motif that is specifically recognized by Cln1 and Cln2, and not by Cln3 or later S- or M-phase cyclins, but the responsible cyclin interface was unknown. Results Here, to explore the role of this new docking mechanism in the cell cycle, we first show that it is conserved in a distinct cyclin subtype (Ccn1). Then, we exploit phylogenetic variation to identify cyclin mutations that disrupt docking. These mutations disrupt binding to multiple substrates as well as the ability to use docking sites to promote efficient, multi-site phosphorylation of substrates in vitro. In cells where the Cln2 docking function is blocked, we observed reductions in the polarized morphogenesis of daughter buds and reduced ability to fully phosphorylate the G1/S transcriptional repressor Whi5. Furthermore, disruption of Cln2 docking perturbs the coordination between cell size and division, such that the G1/S transition is delayed. Conclusions The findings point to a novel substrate interaction interface on cyclins, with patterns of conservation and divergence that relate to functional distinctions among cyclin subtypes. Furthermore, this docking function helps ensure full phosphorylation of substrates with multiple phosphorylation sites, and this contributes to punctual cell cycle entry.

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Section: Resultsmentioning

confidence: 99%

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

et al. 2015

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“…When Cdc28 is associated with Cln3 cyclin, it unfolds the activation of transcriptional G 1 machinery, chiefly through two mechanisms: phosphorylation of the Whi5 repressor (and presumably of Swi6) at multiple residues (10)(11)(12) and control of the Stb1 dual protein and the histone deacetylases (13). In addition to Cln3, other elements involved in G 1 transcription firing have recently been demonstrated: for example, a positive-feedback mechanism involving Cln1 and Cln2 could reinforce SBF/MBF activation (14).…”

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confidence: 99%

Phosphate-Activated Cyclin-Dependent Kinase Stabilizes G₁ Cyclin To Trigger Cell Cycle Entry

Menoyo

Ricco

Bru

et al. 2013

Molecular and Cellular Biology

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G 1 cyclins, in association with a cyclin-dependent kinase (CDK), are universal activators of the transcriptional G 1 -S machinery during entry into the cell cycle. Regulation of cyclin degradation is crucial for coordinating progression through the cell cycle, but the mechanisms that modulate cyclin stability to control cell cycle entry are still unknown. Here, we show that a lack of phosphate downregulates Cln3 cyclin and leads to G 1 arrest in Saccharomyces cerevisiae. The stability of Cln3 protein is diminished in strains with low activity of Pho85, a phosphate-sensing CDK. Cln3 is an in vitro substrate of Pho85, and both proteins interact in vivo. More interestingly, cells that carry a CLN3 allele encoding aspartic acid substitutions at the sites of Pho85 phosphorylation maintain high levels of Cln3 independently of Pho85 activity. Moreover, these cells do not properly arrest in G 1 in the absence of phosphate and they die prematurely. Finally, the activity of Pho85 is essential for accumulating Cln3 and for reentering the cell cycle after phosphate refeeding. Taken together, our data indicate that Cln3 is a molecular target of the Pho85 kinase that is required to modulate cell cycle entry in response to environmental changes in nutrient availability.

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“…Alternatively, the CK2 holoenzyme may be involved in the phosphorylation of different proteins within the transcriptional complex to exert its regulatory activity. This is not surprising considering that also the Whi5-12Ala mutant (with all 12 Cdk1 sites changed to alanine) shows no alteration in cell cycle progression unless it is co-overexpressed with the Swi6-Cdk1 (Swi6-4Ala) phosphorylation mutant (13). Therefore, the CK2 holoenzyme may stimulate gene expression by phosphorylating different key proteins and then acting at several levels of the transcriptional process.…”

Section: Discussionmentioning

confidence: 96%

“…The specific and coherent expression of G 1 -specific genes is achieved by the interaction of SBF and MBF complexes with many different regulators, such as chromatin remodelling factors (Rpd3, Hos3, and the FACT complex), coactivators, and repressors (Stb1 and Whi5) (6)(7)(8)(9)(10)(11)(12)(13). The combined actions of all these proteins allow the recruitment of the mediator complex, the RNA polymerase II complex, and several general transcription factors (GTFs), which ultimately leads to transcription initiation.…”

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confidence: 99%

Protein Kinase CK2 Holoenzyme Promotes Start-Specific Transcription in Saccharomyces cerevisiae

et al. 2013

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In Saccharomyces cerevisiae, the entrance into S phase requires the activation of a specific burst of transcription, which depends on SBF (SCB binding factor, Swi4/Swi6) and MBF (MCB binding factor, Mbp1/Swi6) complexes. CK2 is a pleiotropic kinase involved in several cellular processes, including the regulation of the cell cycle. CK2 is composed of two catalytic subunits (␣ and ␣=) and two regulatory subunits (␤ and ␤=), both of which are required to form the active holoenzyme. Here we investigate the function of the CK2 holoenzyme in Start-specific transcription. The ckb1⌬ ckb2⌬ mutant strain, bearing deletions of both genes encoding CK2 regulatory subunits, shows a delay of S-phase entrance due to a severe reduction of the expression of SBF-and MBF-dependent genes. This transcriptional defect is caused by an impaired recruitment of Swi6 and Swi4 to G 1 gene promoters. Moreover, CK2 ␣ and ␤= subunits interact with RNA polymerase II, whose binding to G 1 promoters is positively regulated by the CK2 holoenzyme. Collectively, these findings suggest a novel role for the CK2 holoenzyme in the activation of G 1 transcription. In the budding yeast Saccharomyces cerevisiae, the entrance into S phase requires the execution of a series of molecular events in the regulatory area called Start (see references 1 and 2 for recent reviews), in which the cell has to activate a specific burst of transcription of about 200 genes (G 1 regulon) involved in bud emergence, DNA synthesis, and spindle pole body duplication (3). Start-specific transcription depends upon two related transcription factors, SBF and MBF, each of which contains the common transcriptional modulator Swi6 and a DNA binding protein, Swi4 in SBF and Mbp1 in MBF. The SBF complex primarily regulates genes involved in cell morphogenesis, spindle pole body duplication, and other growth-related functions, among which are the CLN1 and CLN2 genes. The MBF complex targets genes involved in DNA replication, DNA repair, and metabolism, such as CLB5, CLB6, and RNR1 (4). However, the separation between SBF-and MBF-controlled expression is not absolute, since many genes are regulated by both SBF and MBF complexes (5).The specific and coherent expression of G 1 -specific genes is achieved by the interaction of SBF and MBF complexes with many different regulators, such as chromatin remodelling factors (Rpd3, Hos3, and the FACT complex), coactivators, and repressors (Stb1 and Whi5) (6-13). The combined actions of all these proteins allow the recruitment of the mediator complex, the RNA polymerase II complex, and several general transcription factors (GTFs), which ultimately leads to transcription initiation. Strikingly, many kinases are known to phosphorylate key components of SBF and MBF, such as Cdk1 (14, 15), Pho85 (8), Rad53 (16,17), Slt2 (18,19), and Hrr25 (20). Recently, we showed that protein kinase Snf1/AMPK (AMP-activated protein kinase), which is a central controller of cellular energy and required for responses to different cellular stresses (21), interacts with Swi...

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Whi5 Regulation by Site Specific CDK-Phosphorylation in Saccharomyces cerevisiae

Cited by 70 publications

References 45 publications

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

Phosphate-Activated Cyclin-Dependent Kinase Stabilizes G₁ Cyclin To Trigger Cell Cycle Entry

Protein Kinase CK2 Holoenzyme Promotes Start-Specific Transcription in Saccharomyces cerevisiae

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Whi5 Regulation by Site Specific CDK-Phosphorylation in Saccharomyces cerevisiae

Cited by 70 publications

References 45 publications

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

A Docking Interface in the Cyclin Cln2 Promotes Multi-site Phosphorylation of Substrates and Timely Cell-Cycle Entry

Phosphate-Activated Cyclin-Dependent Kinase Stabilizes G1 Cyclin To Trigger Cell Cycle Entry

Protein Kinase CK2 Holoenzyme Promotes Start-Specific Transcription in Saccharomyces cerevisiae

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Phosphate-Activated Cyclin-Dependent Kinase Stabilizes G₁ Cyclin To Trigger Cell Cycle Entry