The Stress-activated Mitogen-activated Protein Kinase Signaling Cascade Promotes Exit from Mitosis

Vladimír Reiser^*, Katharine E. D’Aquino, Ly-Sha Ee, and Angelika Amon

Center for Cancer Research, Howard Hughes Medical Institute, Massachusetts Institute of Technology, Cambridge, MA 02139

Submitted December 6, 2005; Revised April 17, 2006; Accepted April 21, 2006
Monitoring Editor: Orna Cohen-Fix

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In budding yeast, a signaling network known as the mitotic exitnetwork (MEN) triggers exit from mitosis. We find that hypertonicstress allows MEN mutants to exit from mitosis in a manner dependenton the high osmolarity glycerol (HOG) mitogen-activated protein(MAP) kinase cascade. The HOG pathway drives exit from mitosisin MEN mutants by promoting the activation of the MEN effector,the protein phosphatase Cdc14. Activation of Cdc14 depends onthe Cdc14 early anaphase release network, a group of proteinsthat functions in parallel to the MEN to promote Cdc14 function.Notably, exit from mitosis is promoted by the signaling branchdefined by the Sho1 osmosensing system, but not by the Sln1osmosensor of the HOG pathway. Our results suggest that thestress MAP kinase pathway mobilizes programs to promote completionof the cell cycle and entry into G₁ under unfavorable conditions.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In response to a sudden increase in extracellular osmolarity,cells induce an elaborate program that includes changes in transcriptionand translation as well as cell cycle progression to allow cellsto adapt. Central to this response is a mitogen-activated protein(MAP) kinase signaling pathway known as the high osmolarityglycerol (HOG) pathway in budding yeast and the p38 pathwaysin more complex eukaryotes (reviewed in Hohmann, 2002).

The HOG pathway is composed of the MAP kinase Hog1, its MAPkinase kinase Pbs2 as well as two upstream regulatory branchesthat are defined by two putative osmosensors, Sln1 and Sho1.The Sln1 branch of the pathway is thought to sense changes inturgor pressure (Reiser et al., 2003) through the Ypd1-Ssk1multicomponent phospho-relay system and the redundant Ssk2/Ssk22protein kinases (Posas et al., 1996; Posas and Saito, 1998).The signal sensed by the Sho1 branch is not known but activationof Pbs2 through Sho1 requires proteins that are also involvedin the cells’ response to mating pheromone and includeCdc42, Ste50, Ste20, and Ste11 (Maeda et al., 1995; Posas andSaito, 1997; Raitt et al., 2000; Reiser et al., 2000).

Activation of either the Sln1 or Sho1 branch of the pathwayis sufficient to elicit adaptation to high osmolarity and leadto phosphorylation of Hog1 on strictly conserved T and Y residuesin the catalytic domain of the kinase, thereby activating it.Activated Hog1 then transiently accumulates in the nucleus (Reiseret al., 1999) where it modulates the expression of genes involvedin adaptation to high osmolarity by modulating activity of severaltranscription factors as well as through chromatin remodeling(Rep et al., 1999; Alepuz et al., 2001; Proft and Struhl, 2002;de Nadal et al., 2003, de Nadal et al., 2004). One of the keytranscriptional outputs is the stimulation of intracellularglycerol production, which helps to rebuild the osmotic equilibriumbetween the extracellular and intracellular environment (reviewedin Hohmann 2002).

Activation of the HOG pathway also leads to a transient cellcycle arrest in G₁ or G₂. The transient G₁ arrest is thoughtto be brought about by two mechanisms. First, the HOG pathwaydown-regulates the transcription of key regulators of the G₁–Sphase transition. Cyclin-dependent kinases (Cdc28 in buddingyeast; CDKs) promote entry into the cell cycle when complexedwith Cln1, -2, and -3 cyclin subunits (Cln-CDKs). Activationof the HOG pathway causes inhibition of CLN1 and CLN2 transcriptionby an unknown mechanism (Escote et al., 2004). Second, Hog1directly phosphorylates an inhibitor of DNA replication, Sic1,thereby preventing the protein’s degradation and entryinto DNA replication (Escote et al., 2004). Activation of theHOG pathway also delays cell cycle progression in G₂ (Alexanderet al., 2001) by inhibiting the mitosis-inducing Clb-CDKs transcriptionallyand posttranscriptionally. How HOG pathway activation leadsto inhibition of CLB cyclin transcription and activation ofSwe1, which inhibits Clb-CDKs is unknown.

Hypertonic stress also seems to regulate exit from mitosis,the cell cycle transition from mitosis into G₁. The failureof certain mutants to execute this transition can be suppressedby a high osmotic environment (Grandin et al., 1998). Exit frommitosis is triggered by the protein phosphatase Cdc14, whichbrings about this cell cycle transition by antagonizing Clb-CDKs(reviewed in Stegmeier and Amon, 2004). The protein phosphataseitself is tightly regulated by a competitive inhibitor Cfi1/Net1.The inhibitor holds Cdc14 inactive in the nucleolus during G₁phase, S phase, and early mitosis. During anaphase, Cdc14 isreleased from its inhibitor and spreads throughout the nucleusand cytoplasm to induce exit from mitosis. The release of Cdc14from its inhibitor is brought about by two regulatory networks,the Cdc14 early anaphase release (FEAR) network and the mitoticexit network (MEN). The FEAR network promotes Cdc14 activationduring early anaphase but is not essential for Cdc14 to promoteexit from mitosis. The MEN functions during later stages ofanaphase to activate Cdc14. This pathway’s Cdc14-promotingfunctions are essential for exit from mitosis to occur. Cellscarrying temperature-sensitive mutations in components of theMEN arrest in late anaphase, with Cdc14 sequestered in the nucleolus.The cell cycle arrest of two temperature-sensitive MEN mutants,cdc15-2 and dbf2-2 has been shown to be partially suppressedby a high osmotic environment (Grandin et al., 1998). The mechanismunderlying this suppression was unknown.

Here, we show that hypertonic stress allows MEN mutants to releaseCdc14 from the nucleolus and to exit from mitosis in a mannerdependent on the HOG MAP kinase cascade. Release of Cdc14 fromits inhibitor depends on the FEAR network, suggesting that theHOG pathway regulates the FEAR network or functions in parallelto it to promote exit from mitosis in MEN mutants. Interestingly,exit from mitosis is promoted by the signaling branch definedby the Sho1 osmosensing system but not by the Sln1 branch ofthe HOG pathway. Our results suggest that the stress MAP kinasepathway promotes completion of the cell cycle and entry intoG₁ in a hypertonic environment and defines the first extracellularsignal regulating Cdc14 and exit from mitosis.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Strains
All strains are derivative of W303 (K699). Deletions of geneswere performed by the PCR-based method described in Longtineet al. (1998).

Cell Synchronization
Cells were arrested in G₁ in YPD medium containing 5 µg/ml ${alpha}$ -factor and subsequently released into ${alpha}$ -factor-free YPD mediumat 37°C. To release cells from a nocodazole block, cellswere first arrested by addition of 15 µg/ml nocodazole(1% dimethyl sulfoxide [DMSO]) in YPD medium for 2–3 hand then washed and released into fresh YPD containing 1% DMSO.To avoid activation of the HOG pathway by heat shock, the followingregimen was used to shift temperature-sensitive mutants to therestrictive temperature. Cells were grown at 25°C and thenwashed and resuspended in medium and placed into a water-bathshaker that has been set to 30°C. The temperature of thewater bath was then raised gradually to reach 37°C withina 10- to 15-min time interval. Sorbitol was prewarmed to 37°Cbefore adding to cells.

Microscopy
Immunofluorescence (tubulin, Myc-tagged Dbf2, and hemagglutinin[HA]-tagged Cdc14), fluorescence (SPC42-cyan fluorescent protein[CFP]), and light microscopy techniques were as described previouslyin Visintin et al. (1999) and Visintin and Amon (2001). Imageswere captured using an Axioplan 2 microscope (Carl Zeiss, Thornwood,NY) and analyzed using the Openlab software package (Improvision,Lexington, MA). Cell viability was determined using the LIVE/DEADyeast viability assay manufactured by Invitrogen (Carlsbad,CA).

Protein Techniques
Western blot analysis and Dbf2 and Clb2 kinase assays were performedas described previously (Visintin and Amon, 2001). The followingantibodies were used: anti-HA (HA-11; BAbCO, Richmond, CA),anti-myc (9E10; BAbCO), anti- ${alpha}$ -tubulin (Oxford Biotechnology,Kidlington, United Kingdom), and anti-Hog1 antibodies (SantaCruz Biotechnology, Santa Cruz, CA). Hog1 phosphorylation wasmeasured using an anti-phospho-p38 antibody (Cell SignalingTechnology, Beverly, MA).

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

A Hypertonic Environment Suppresses the Proliferation Defect of Temperature-sensitive MEN Mutants
Temperature-sensitive mutants in the MEN components CDC15, TEM1,and DBF2 arrest in anaphase due to a failure to inactivate Clb-CDKs,and as a consequence, cells do not exit from mitosis. However,when grown in hypertonic medium, such as YPD supplemented withsorbitol or sodium chloride, temperature-sensitive MEN mutantswere able to proliferate (Figure 1A;Grandin et al., 1998). Ahypertonic environment did not allow cells deleted for MEN componentsto proliferate (our unpublished data), indicating that someMEN activity was necessary for high osmolarity to bring aboutexit from mitosis. The suppression of the temperature-sensitivelethality by high osmolarity was nevertheless specific to MENmutants because the proliferation defect of other temperature-sensitivecell cycle mutants was not suppressed by a hypertonic environment(Table 1).

View larger version (30K):
[in this window]
[in a new window]

Figure 1. A hypertonic environment rescues the mitotic exit defect of MEN mutants. (A) Strains carrying temperature-sensitive alleles of genes encoding components of the MEN were spotted on solid media supplemented with sorbitol or NaCl. Strains used (from top) are A1411, A1740, A1674, A851, A5321, and A859. Note that the cdc5-1 strain was sensitive to 0.5 M NaCl. (B) A hypertonic environment does not accelerate exit from mitosis: wild-type cells were arrested with 15 µg/ml nocodazole followed by release from the block in the presence or absence of 1.5 M sorbitol. The percentage of cells with metaphase and anaphase spindles was determined at the indicated times. Note that all cells were arrested by the nocodazole treatment. However, upon washout of the drug (0 time point), repolymerization of metaphase spindles is sluggish leading to only 30–50% of cells having reformed metaphase spindles at the beginning of the time course.

View this table:
[in this window]
[in a new window]

Table 1. Suppression of various temperature-sensitive cell cycle mutants by high osmolarity at restrictive temperature

In contrast to MEN mutants, strains carrying temperature-sensitivemutations in the MEN effector CDC14 (Shou et al., 1999

; Visintinet al., 1999

) were not able to grow under hypertonic cultureconditions. Cells bearing either the cdc14-1 or cdc14-3 allelefailed to proliferate in sorbitol-containing medium at 37°C(Figure 1A and Table 1). A previous report (Grandin et al.,1998

) mentioned that high osmolarity suppressed the temperature-sensitivegrowth defect of cdc14-1 mutants. The reason for this discrepancyis at present unclear.

SIC1, which encodes an inhibitor of Clb-CDKs, and CDH1, whichfunctions as an activator of Clb cyclin degradation, are criticaltargets of CDC14 in promoting exit from mitosis (reviewed inStegmeier and Amon, 2004). Deletion of either gene preventedcdc15-2 mutants to proliferate at 37°C in the presence ofsorbitol (Table 1). Furthermore the lethality associated withthe expression of a Clb2 mutant that cannot be degraded wasnot suppressed by hypertonic growth conditions (our unpublisheddata). Together, these results indicate that CDK inactivationis required for high osmolarity to promote proliferation ofMEN mutants. Our results suggest that a hypertonic environmenteither restores signaling through the MEN or promotes Cdc14activity and Clb-CDK inactivation by a parallel mechanism.

To examine whether a hypertonic environment also affects thekinetics of exit from mitosis during an unperturbed cell cycle,we analyzed the effects of 1.5 M sorbitol on wild-type cellsexiting mitosis upon release from a nocodazole-induced metaphasearrest. Cells treated with sorbitol progressed through mitosisless efficiently than untreated cells, but the kinetics of exitfrom mitosis was similar under both culture conditions (Figure 1B).Furthermore, exit from mitosis upon release from a MEN mutantblock was also not accelerated by addition of sorbitol to themedium (our unpublished data). These results indicate that ahypertonic environment cannot accelerate exit from mitosis whenthis cell cycle transition occurs with wild-type kinetics. Thus,the exit from mitosis promoting function of a hypertonic environmentis only revealed when cell cycle progression is halted or delayedin anaphase.

The Suppression of MEN Mutants by High Osmolarity Is Not Due to Increased Glycerol Production
To investigate whether the rescue of the temperature-sensitivegrowth defect of MEN mutants by high osmolarity was due to anincrease in intracellular glycerol levels that occurs in responseto a high osmotic environment (reviewed in Hohmann, 2002), weexamined the consequences of deleting GPD1. GPD1 encodes themajor NAD-dependent glycerol-3-phosphate dehydrogenase thatis responsible for glycerol accumulation in response to an increasein the osmotic environment (Albertyn et al., 1994). Deletionof GPD1 reduced the ability of MEN mutants to grow on mediumcontaining sorbitol to the same extent as that of wild-typecells (our unpublished data). Several other observations furtherargue against the idea that an increase in intracellular glycerolis responsible for the suppression of the temperature-sensitivelethality of MEN mutants by high osmolarity. First, overexpressionof GPD1 did not promote proliferation of MEN mutants that weredefective in the HOG pathway component PBS2 (our unpublisheddata). Second, overexpression of the HOG pathway component STE20rescued the temperature-sensitive growth defect of cdc15-2 mutantsin a GPD1-independent manner (Figure 7C). Finally, inactivationof the osmosensor SHO1 prevents cdc15-2 mutants to exit frommitosis and to grow at 37°C in the presence of sorbitol(Figure 7, A and B), yet GPD1 induction and osmoresistance arenot affected by deleting SHO1 (Figure 7A; Maeda et al., 1995;O’Rourke and Herskowitz, 2004). Together, these resultsindicate that an increase in intracellular glycerol levels isneither required nor sufficient for the rescue of MEN mutantsby high osmolarity.

The Suppression of MEN Mutants by Hypertonic Treatment Depends on HOG Pathway Function
In budding yeast, hypertonic stress activates the HOG pathway(reviewed in Hohmann, 2002). We found that suppression of theproliferation defect of MEN mutants by a hypertonic environmentdepended on this MAP kinase signaling cascade. Transfer to ahypertonic environment allowed cdc15-2 cells to exit from mitosisand enter the next cell cycle as judged by their ability toduplicate spindle pole bodies (Figure 2A) and to form new buds(Figure 2B).

View larger version (54K):
[in this window]
[in a new window]

Figure 2. The HOG pathway drives exit from mitosis in MEN mutants in response to hypertonic stress. (A) Budding pattern as well as SPB number and distribution were analyzed in cdc15-2 (A9943) cells arrested in anaphase at restrictive temperature before (–Sorb) and 60 min after (+Sorb) addition of 1.5 M sorbitol. SPB number and distribution was monitored using CFP fused to the SPB protein Spc42 (localization indicated by white arrows). (B) cdc15-2 (A1674) and cdc15-2 pbs2 ${Delta}$ (A10710) cells were arrested in anaphase at 37°C (0-min time point), treated with 1.5 M sorbitol and then examined at the indicated time points by light microscopy using a DIC filter. (C) Wild-type (A1411) and pbs2 ${Delta}$ (A9610) cells were arrested in mitosis with nocodazole at 37°C. When the arrest was complete (after 150 min), cells were released from the block in the presence of 1.5 M sorbitol at 37°C, and the percentage of cells with small buds was determined. (D) cdc15-2 (A1674) and cdc15-2 pbs2 ${Delta}$ (A10710) cells were analyzed for their metabolic activity and cell wall integrity before and 150 min after osmotic stress (1.5 M sorbitol) at 37°C. The percentage of viable cells is indicated for each strain and conditions. (E) cdc15-2 (A1674) cells were arrested at 37°C for two hours. When the arrest was complete the culture was split, and one-half of the culture was maintained at 37°C and the other half was transferred into medium containing 1.5 M sorbitol. At the same time, 5 µg/ml ${alpha}$ -factor was added to prevent sorbitol-treated cells from entering the next cell cycle. At the indicated times, samples were taken to determine the total amount of Clb2 and Sic1 protein as well as Clb2 kinase activity.

To determine whether the exit from mitosis observed in cdc15-2mutants in the presence of sorbitol was associated with theinactivation of Clb-CDKs, we measured Clb2-associated kinasesactivity as well as Clb2 cyclin and Sic1 levels, all markersfor exit from mitosis (reviewed in Stegmeier and Amon, 2004

).Because exit from mitosis brought about by sorbitol does notoccur very synchronously ${alpha}$ -factor pheromone was added at thetime of sorbitol addition to arrest cells in G₁ when Clb-CDKactivity is low. Sic1 accumulation and Clb2-CDK inactivationwas observable 90 and 120 min after sorbitol addition, respectively(Figure 2E). Clb2 cyclin degradation was not as obvious andonly started to occur at the last time point. Why Clb2 degradationis not occurring earlier is at present unclear. Our resultsnevertheless indicate that the exit from mitosis in cdc15-2mutants caused by sorbitol is accompanied by Clb-CDK inactivation.

Next, we determined whether an intact HOG pathway was requiredfor a hypertonic environment to induce exit from mitosis inMEN mutants. cdc15-2 mutants lacking the HOG pathway MAPKK encodinggene PBS2 failed to exit from mitosis and to form new buds (Figure 2B).This failure to exit from mitosis was not simply due to cellslacking PBS2 to proliferate in a high osmotic environment. pbs2 ${Delta}$ cells formed new buds when released from a mitotic arrest inducedby nocodazole in the presence of 1.5 M sorbitol (Figure 2C),and cells retained high viability (Figure 2D). Furthermore,deletion of SHO1, which does not impair proliferation underhypertonic conditions (Maeda et al., 1995), also prevented cdc15-2mutants to exit from mitosis in the presence of sorbitol (Figure 7B).We conclude that an intact HOG pathway is necessary for hypertonicstress to bring about exit from mitosis in cdc15-2 mutants.

The Hog1 MAP kinase is activated only transiently in responseto hypertonic stress and its activity returns to prestress levelswithin 20 min after exposure to hypertonic conditions at 30°C(Brewster et al., 1993; Maeda et al., 1995). How is it possiblethat this transient activation supports continuous proliferationof MEN mutants? We observed that conditions that rescued MENmutants (1.5 M sorbitol at 37°C) significantly lengthenedHOG pathway activation as judged by the persistence of dualT174, Y176 phosphorylation on Hog1 in both wild-type and cdc15-2strains (Figure 7D). Our results indicate that sustained activationof the HOG pathway allows MEN mutants to proliferate at therestrictive temperature.

Hypertonic Conditions Promote Cdc14 Release from the Nucleolus in MEN Mutants
The MEN stimulates exit from mitosis by promoting the dissociationof the protein phosphatase Cdc14 from its inhibitor Cfi1/Net1in the nucleolus (Shou et al., 1999; Visintin et al., 1999).In the absence of MEN function, cells arrest in anaphase withCdc14 sequestered in the nucleolus. To determine whether exitfrom mitosis in MEN mutants brought about by HOG pathway activationwas associated with the release of Cdc14 from the nucleolus,we analyzed cell cycle progression in cdc15-2 and cdc15-2 pbs2 ${Delta}$ mutants in detail. Cells were synchronized in G₁ and releasedinto the cell cycle at the restrictive temperature. When 80%of cdc15-2 mutants were arrested in anaphase, sorbitol (1.5M) was added. Cdc14 seemed released from the nucleolus immediatelyafter sorbitol addition in cdc15-2 cells (Figure 3, G and H)and anaphase spindle disassembly occurred (Figure 3, B, C, andF). Cells then entered the next cell cycle as judged by theirability to form new buds and metaphase spindles (Figures 2Band 3, C and F). Cdc14 was also initially released from thenucleolus in 60% of cdc15-2 pbs2 ${Delta}$ cells but was then found resequesteredin the nucleolus within 20 min (Figure 3I). Anaphase spindlesalso disassembled in 40% of cdc15-2 pbs2 ${Delta}$ cells (Figure 3, Dand F), but cells never exited mitosis and entered the nextcell cycle as judged by their inability to form new buds andmetaphase spindles (Figures 2B and 3D). Curiously, after prolongedincubation periods (260-min time point) anaphase spindles seemedto reform in cdc15-2 pbs2 ${Delta}$ cells (Figure 3, E and I). Cdc14 wasalso released from the nucleolus and exit from mitosis occurredin cdc15-2 mutants treated with NaCl (Figure 4). However, incontrast to sorbitol treatment addition of NaCl did not promotethe dissociation of Cdc14 from the nucleolus in cdc15-2 pbs2 ${Delta}$ cells (Figure 4) further indicating that the transient releaseof Cdc14 from the nucleolus observed in sorbitol treated cdc15-2pbs2 ${Delta}$ cells is due to a transient disruption of the nucleolus.

View larger version (47K):
[in this window]
[in a new window]

Figure 3. The HOG pathway promotes Cdc14 release from the nucleolus in MEN mutants treated with sorbitol. cdc15-2 (A1674) and cdc15-2 pbs2 ${Delta}$ (A10710) cells were arrested in G₁ with ${alpha}$ -factor and released from the block at 37°C. The percentage of cells with metaphfase and anaphase spindles (A–E) or Cdc14 release from the nucleolus in anaphase cells (H and I) was scored at the indicated times. Sorbitol (C, D, H, and I) or sorbitol and cycloheximide (1 mg/ml) (E) was added 120 min after release from the G₁ arrest (0-time point, indicated by the orange arrow) with the exception of the control strains (A and B). Hyperosmotic stress stimulates the appearance of metaphase spindles (tubulin staining) in cdc15-2, but not in cdc15-2 pbs2 ${Delta}$ mutants (F) and release of Cdc14 from the nucleolus (G) at the restrictive temperature. Note that in contrast to anaphase spindles, metaphase spindles do not seem to be sensitive to sorbitol treatment. Spindle depolymerization upon sorbitol addition did not occur in cdc13-1 (A2598; our unpublished data).

View larger version (20K):
[in this window]
[in a new window]

Figure 4. The HOG pathway promotes Cdc14 release from the nucleolus in MEN mutants treated with NaCl. cdc15-2 (A1674) and cdc15-2 pbs2 ${Delta}$ (A10710) cells were arrested at 37°C for 2 h. When the arrest was complete, the cdc15-2 culture was split, and one-half of the culture was maintained at 37°C and the other half was transferred into medium containing 0.5 M NaCl. The cdc15-2 pbs2 ${Delta}$ culture was transferred to 37°C medium containing 0.5 M NaCl. At the indicated times, samples were taken to determine the percentage of cells with small buds (A) and the release of Cdc14 from the nucleolus (B). The graph on the left in B shows the percentage of cdc15-2 cells with Cdc14 released from the nucleolus in medium lacking NaCl. The graph in the middle shows the percentage of cdc15-2 cells with Cdc14 released from the nucleolus in medium containing NaCl. The graph on the right shows the percentage of cdc15-2 pbs2 ${Delta}$ cells with Cdc14 released from the nucleolus in medium containing NaCl. "Partial release" is defined as some Cdc14 being diffuse throughout the cell, but some enrichment of Cdc14 being detectable in the nucleolus.

Our results indicate that in the presence of sorbitol, releaseof Cdc14 from the nucleolus is biphasic in cdc15-2 cells withno significant difference between the cdc15-2 and the cdc15-2pbs2 ${Delta}$ strain during the initial phase of the Cdc14 release (Figure 3,H and I; 140-min time point). However, the second wave of Cdc14release from the nucleolus depends on the HOG pathway. We believethat the first HOG pathway-independent wave of Cdc14 loss fromthe nucleolus reflects high osmolarity-induced disturbancesof the nucleolar compartment and in consequence redistributionof Cdc14 bound to its inhibitor, rather than the dissociationof Cdc14 from its inhibitor and hence its activation. This conclusionis supported by two findings. First, cdc15-2 pbs2 ${Delta}$ cells do notexit from mitosis (Figure 3E). Second, in agreement with previousfindings (Nanduri et al., 2001

), we also observed that the nucleolarprotein Nop1 (Schimmang et al., 1989

) temporarily diffused (forup to 60 min) throughout the cell after sorbitol addition at37°C (our unpublished data). The disassembly of the mitoticspindle in 40% of cdc15-2 pbs2 ${Delta}$ cells also did not reflect exitfrom mitosis, as entry into a new cell cycle did not occur (Figure 3,A and E). Instead, spindle disassembly is likely to be causedby a sensitivity of anaphase spindles to mechanical stress imposedby cell volume shrinkage (Reiser et al., 2003

) during the initialexposure to hypertonic conditions. Consistent with this ideais the observation that a similar collapse of anaphase spindlesoccurred in the cdc14-3 mutant, whose proliferation defect wasnot rescued by a hypertonic environment (our unpublished data).The disassembly of the mitotic spindle in 40% of cdc15-2 pbs2 ${Delta}$ cells also shows that anaphase spindle disassembly cannot beused as a marker for exit from mitosis when examining the effectsof osmotic stress on MEN mutants. Rather, the formation of newbuds and of metaphase spindles must be used as an indicatoras to whether or not exit from mitosis had occurred.

In summary, our results revealed two responses of MEN mutantsto sorbitol treatment. A transient HOG pathway-independent responsethat leads to a temporary disruption of nuclear and nucleolarstructures and a sustained, HOG pathway-dependent response thatleads to the suppression of the mitotic exit defect of MEN mutants.Our results further indicate that the HOG pathway promotes exitfrom mitosis by inducing Cdc14 release from the nucleolus. Thisrelease likely requires the transcriptional response inducedby the HOG pathway, because it did not occur in the presenceof the translation inhibitor cycloheximide (Figure 3E) and dependedon the chromatin remodeling factors Rpd3 and Sin3, which arenecessary for the transcriptional induction of HOG pathway-responsivegenes (de Nadal et al., 2004; Figure 7A).

The FEAR Network Is Required for Hypertonic Treatment to Promote Exit from Mitosis in MEN Mutants
How does activation of the HOG pathway promote Cdc14 releasefrom the nucleolus and exit from mitosis in MEN mutants? Weknow of two pathways, the mitotic exit and FEAR networks thatpromote the dissociation of Cdc14 from its inhibitor in thenucleolus during anaphase. To test whether high osmolarity restoressignaling to MEN mutants, we first examined the localizationand activity of Dbf2 kinase in cdc15-2 mutants treated withsorbitol. DBF2 is the most downstream component of the MEN identifiedto date. Upon MEN activation Dbf2 associates with spindle polebodies (SPBs) and becomes active as a kinase (Visintin and Amon,2001). As reported previously (Visintin and Amon, 2001), Dbf2did not localize to SPBs, and kinase activity was low in cdc15-2mutants (Figure 5, A and B). Addition of sorbitol to cdc15-2mutants allowed Dbf2 to associate with SPBs in 25% of cells(Figure 5B) but did not lead to detectable amounts of Dbf2 kinaseactivity (Figure 5A). This result together with the findingthat the HOG pathway cannot promote exit from mitosis in cellsdeleted for MEN components suggests that some level of MEN signaling,though too low to detect by in vitro Dbf2 kinase assays, isimportant for the HOG pathway to promote exit from mitosis.

View larger version (56K):
[in this window]
[in a new window]

Figure 5. The FEAR network is required for the suppression of MEN mutants by high osmolarity. (A) A hypertonic environment does not increase the activity of the MEN kinase Dbf2. cdc15-2 (A2096) cells were arrested at the nonpermissive temperature (0 min), treated with sorbitol (1.5 M) with or without cycloheximide (1 mg/ml), and then assayed for Dbf2 kinase activity at indicated times using histone H1 as a substrate. As a control, Dbf2 kinase activity was measured in wild-type cells (A2747 arrested in G₁ [G₁] and in wild-type cells that were in anaphase [Ana]). Anaphase cells were obtained by first synchronizing cells in G₁ and then releasing cells from the G₁ block. Cells were harvested when >90% of cells were in anaphase. (B) cdc15-2 cells carrying a Dbf2-Myc fusion (A2096) were arrested at 37°C for 2 h. When the arrest was complete the culture was split, and one-half of the culture was maintained at 37°C and the other half was transferred into medium containing 1.5 M sorbitol. At the indicated times samples were taken to determine the localization of Dbf2 at SPBs. (C) Cells (from top: A1674, A6895, and A12435) all carrying SPO12 under the control of the GAL1-10 promoter were spotted onto plates containing galactose at either 25 or 37°C. (D) cdc15-2 mutants carrying mutations in FEAR network components fail to grow on plates containing 1.5 M sorbitol. Strains were spotted on plates with or without sorbitol. Strains used (from top) are A1411, A1674, A4168, and A10010. (E) cdc15-2 mutants (A1674) and cdc15-2 spo12 ${Delta}$ mutants (A10408) were arrested in G₁ with ${alpha}$ -factor and released from the block at 37°C. Sorbitol was added 120 min after release from the G₁ arrest (0-time point), and the localization of Cdc14 in anaphase cells was examined.

Next, we tested whether Cdc14 release from the nucleolus andexit from mitosis in MEN mutants brought about by the HOG pathwayrequired the FEAR network. Components of the FEAR network suchas Spo12 or Cdc5 can, when overproduced, suppress the temperature-sensitivelethality of MEN mutants (Parkes and Johnston, 1992

; Jaspersenet al., 1998

; Stegmeier et al., 2002

). We found that overexpressionof SPO12 suppressed the proliferation defect of cdc15-2 mutantsas well as of cdc15-2 pbs2 ${Delta}$ mutants (Figure 5C). Furthermore,cdc15-2 mutants lacking the FEAR network components SPO12 orSLK19 were no longer able to proliferate under hypertonic cultureconditions at 37°C (Figure 5D), and Cdc14 release inducedby high osmolarity was lost in the cdc15-2 spo12 ${Delta}$ double mutant(Figure 5E). These results indicate that the HOG pathway requiresthe FEAR network to suppress the mitotic exit defect of MENmutants. Thus, the HOG pathway either functions upstream ofor in parallel to the FEAR network to promote exit from mitosiswhen the MEN is impaired.

The HOG Pathway Contributes to Exit from Mitosis under Nonstress Conditions
The HOG pathway could promote exit from mitosis only in responseto hypertonic conditions or function during every cell cycleunder nonstress conditions to promote exit from mitosis. Todistinguish between these possibilities, we analyzed the localizationof Cdc14 in cells lacking HOG1 or PBS2 during an unperturbedcell cycle. Deletion of either MAP kinase cascade componenthad no effect on Cdc14 localization either at 25 or 37°C(Figure 6A). However, deletion of the HOG pathway componentsHOG1, PBS2, or STE20 reduced the restrictive temperature ofcdc15-2 mutants (Figure 6B) and led to a synthetic growth defectwhen combined with a deletion in the MEN activator LTE1 (Figure 6C;Hofken and Schiebel, 2002; note that the growth defect of lte1 ${Delta}$ ste20 ${Delta}$ double mutants is more severe than that of lte1 ${Delta}$ pbs2 ${Delta}$ orlte1 ${Delta}$ hog1 ${Delta}$ mutants, which indicates that STE20 has functionsin addition to HOG pathway signaling during exit from mitosis).Our results indicate that the HOG pathway contributes to theregulation of exit from mitosis under nonstress conditions.

View larger version (43K):
[in this window]
[in a new window]

Figure 6. The HOG pathway promotes exit from mitosis under nonstress conditions. (A) Wild-type (A1411) and pbs2 ${Delta}$ (A9610) strains were released from a pheromone-induced G₁ arrest and the percentage of cells with anaphase spindles (ana) and Cdc14 released from nucleolus (Cdc14) was determined at the indicated times. (B) Mutations in the HOG pathway enhance the temperature sensitivity of cdc15-2 mutants. Strains were spotted on YPD plates and cultured at the indicated temperatures. Strains used (from the top left, CDC15) are A1674, A9610, A9608, and A11812 (CDC15) and (from the top right, cdc15-2) A1674, A10710, A10707, and A11813 (cdc15-2). (C) Mutations in the HOG pathway enhance the proliferation defect of lte1 ${Delta}$ cells. Serial dilutions of strains with the indicated genotype and carrying an LTE1-URA3 plasmid were spotted on YPD and on plates containing 5'-fluoroorotic acid (5-FOA). Strains used (from the top) are A4101, A6307, A12253, and A12254.

The Sho1 Branch of the HOG Pathway Promotes Exit from Mitosis in MEN Mutants
The HOG pathway consists of two branches, each defined by atransmembrane protein at the top of the pathway. Although inactivationof both the Sln1 and Sho1 branch is necessary to eliminate theresponse to osmotic stress, it is thought that the two branchesof the pathway respond to different signals. Turgor pressureis thought to activate the Sln1 branch (Reiser et al., 2003

).An osmotic signal controlling the Sho1 branch of the pathwayhas not been identified.

We examined the ability of hypertonic conditions to suppressthe proliferation defect of cdc15-2 mutants in the absence ofcomponents of the two HOG pathway branches. Whereas the cdc15-2ssk1 ${Delta}$ strain (the SLN1 branch is inactive) displayed a similarproliferation rate as a cdc15-2 strain in the presence of sorbitolat the restrictive temperature (Figure 7A), the cdc15-2 sho1 ${Delta}$ mutant neither exited mitosis in the presence of sorbitol asjudged by the formation of small buds (Figure 7B), nor did itform colonies on plates containing sorbitol (Figure 7A). cdc15-2cells deleted for either STE20 or STE11, both of which encodeprotein kinases acting in the Sho1 branch of the HOG pathwaydid not proliferate either (Figure 7A). Furthermore, we foundthat overexpression of STE20 was able to alleviate the growthdefect of cdc15-2 mutants (Figure 7C). This suppression dependedon downstream components in the HOG pathway (PBS2, HOG1, RPD3,and SIN3) as well as the FEAR network components SLK19 and SPO12(Figure 7C). These data indicate that the Sho1 branch of theHOG pathway is responsible for promoting exit from mitosis inMEN mutants. Consistent with this idea was the observation thatactivation of the SHO1 branch in cdc15-2 mutants in responseto hypertonic stress occurred over an extended period, whichwas in stark contrast to the transient activation of the SLN1branch (Figure 7D). Our results demonstrate an essential rolefor the Sho1 branch of the HOG pathway in promoting mitoticexit in MEN mutants after osmotic stress and advocate for afunctional diversification between individual signaling branchesof the HOG pathway in osmoprotection.

View larger version (66K):
[in this window]
[in a new window]

Figure 7. Suppression of the temperature-sensitive growth defect of MEN mutants by high osmolarity depends on the Sho1 signaling branch of the HOG pathway. (A) The Sho1 branch, but not the Sln1 branch of the HOG pathway, is necessary for the high osmolarity-induced suppression of MEN mutants. Strains were spotted onto media with or without 1.5 M sorbitol. Strains used (from the top, the CDC15+ strain is noted first) are A2587, A1674, A11678, A11681, A11812, A11813, A5816, A8353, A11679, A11682, A11680, A11683, A9610, A10710, A9608, A10707, A11572, A11573, A11576, and A11577. (B) cdc15-2 (A1674) and cdc15-2 sho1 ${Delta}$ (11683) cells were arrested at 37°C for 2 h. When the arrest was complete, cells were transferred into medium containing 1.5 M sorbitol. At the indicated times, samples were taken to determine the percentage of cells with small buds. (C) Cells carrying a multicopy plasmid containing STE20 were grown on YPD plates at the indicated temperatures. Strains used (from the top) are A1674, A12227, A12228, A12229, A12230, A12231, A12232, A12233, A12227, and A14535. (D) Activation of Hog1 in cdc15-2 strains in response to osmotic stress. cdc15-2 cells were arrested at 37°C. After 2 h (0-time point), 1.5 M sorbitol was added. Samples were taken at the indicated times to determine Hog1 activity using an antibody that recognizes double phosphorylation of the TGY amino acid motif in Hog1. The total amount of Hog1 was determined using an anti-Hog1 antibody. Signals were quantified and normalized to protein levels of Hog1 (graph). Strains used (from the top) are A1411, A1674, A11682, and A11681.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Here, we show that hypertonic stress allows mutants defectiveor compromised in exit from mitosis to traverse this cell cycletransition. Mutants compromised in other cell cycle transitionsare not rescued by a hypertonic environment, suggesting a specificeffect of high osmolarity on mutants defective in exit frommitosis. The suppression of the mitotic exit defects of MENmutants by high osmolarity is accompanied by the release ofCdc14 from the nucleolus and is mediated by the HOG pathway,indicating that the HOG pathway brings about exit from mitosisin MEN mutants by promoting the release of Cdc14 from its inhibitorin the nucleolus. Finally, we find that only one of the twobranches of the HOG pathway, the Sho1 branch of the pathway,is required for promoting exit from mitosis in MEN mutants,which, to our knowledge, represents the first specific functionfor the Sho1 branch of the HOG pathway.

The Effects of High Osmolarity and Its MAP Kinase Pathway on Exit from Mitosis
The effects of osmotic stress on exit from mitosis only becomeapparent in cells with reduced MEN activity, i.e., in temperature-sensitiveMEN mutants or cells defective for the MEN activator LTE1. Themitotic exit promoting activities of a hypertonic environmentwere not observed in an unperturbed cell cycle indicating thathigh osmolarity does not accelerate exit from mitosis when thiscell cycle transition occurs with wild-type kinetics. Does thismean that the suppression of MEN mutants by the HOG pathwayis the result of pleiotropic nonspecific effects of HOG pathwaystimulation? We think it does not. Our results indicate thatan increase in intracellular glycerol levels, which could leadto suppression of temperature-sensitive mutants, was not responsiblefor the suppression of MEN mutants. Furthermore, it is importantto note that it is not trivial to accelerate exit from mitosisin wild-type cells. Only severe overproduction of Cdc5 (Visintinet al., 2003) or of a dominant active form of Cdc15 (Bardinet al., 2003) can accomplish this. This is probably not surprisingbecause multiple layers of control govern this cell cycle transition,and other pathways are likely to prevent the HOG pathway fromaccelerating exit from mitosis. Only when MEN activity is compromisedis the positive regulatory role of the HOG pathway revealed.

Another key question is whether the HOG pathway promotes exitfrom mitosis only in response to hypertonic conditions or whetherit also functions under nonstress conditions to induce exitfrom mitosis. Although inactivation of HOG1 or PBS2 did notaffect exit from mitosis or Cdc14 localization during an unperturbedcell cycle, two observations point to the MAP kinase pathwaycontributing to promoting exit from mitosis under nonstressconditions. Deletion of HOG pathway components reduces the restrictivetemperature of MEN mutants and leads to a synthetic growth defectwhen combined with a deletion of LTE1. Thus, our results suggestthat—although not essential for promoting exit from mitosis—theHOG pathway contributes to exit from mitosis under nonstressconditions, which becomes apparent when MEN activity is compromised.

The HOG Pathway Regulates Cdc14 Localization
The HOG pathway seems to bring about exit from mitosis in MENmutants by activating Cdc14. The mitotic exit observed in MENmutants upon transfer of cells to a hypertonic environment isaccompanied by the release of Cdc14 from the nucleolus. Thisrelease solely depends on the HOG pathway when cells are challengedwith NaCl and is biphasic when cells are challenged with sorbitol.In the latter case, we observe that the initial wave of Cdc14release is independent of the HOG pathway and not capable ofpromoting exit from mitosis. We therefore think that this releaseof Cdc14 from the nucleolus does not actually reflect the dissociationof Cdc14 from its inhibitor and thus Cdc14 activation but rathera transient disruption of nucleolar structures due to the suddenchanges in osmolarity (Nanduri and Tartakoff, 2001). The secondmode by which Cdc14 is released from the nucleolus in responseto sorbitol addition depends on the HOG pathway and reflectsgenuine activation of Cdc14. It is accompanied by exit frommitosis and is followed by entry into the next cell cycle.

Which aspects of HOG pathway signaling are important for itsrole in releasing Cdc14 from the nucleolus and in promotingexit from mitosis? Suppression of MEN mutants by high osmolarityrequires the transcriptional program induced by the HOG pathway.The expression of many genes is modulated upon HOG pathway activation(O’Rourke and Herskowitz, 2004), making the identificationof effector(s) that regulate mitotic exit in response to HOGpathway activation difficult. However, clear predictions canbe made concerning their characteristics. First, genes thatbring about exit from mitosis in MEN mutants ought to be induced(in case they are activators of mitotic exit) or inhibited (incase they are inhibitors of exit from mitosis) by high osmolarityin MEN mutants at 37°C. Second, transcription of this factor(s)should be affected by the deletion of SHO1 but not by deletionof components of the Sln1 branch of the pathway.

The transcriptional response induced by the HOG pathway ultimatelyimpinges on regulators of Cdc14 localization. Our results showthat suppression of the MEN mutants by high osmolarity not onlyrequires the HOG pathway but also MEN activity. Although wedo not detect stimulation of Dbf2 kinase activity by high osmolarity,sorbitol addition cannot promote exit from mitosis in cellsdeleted for MEN components. Do these findings then mean thathigh osmolarity directly affects MEN signaling? Although possiblewe favor the idea that the HOG pathway functions in parallelto the MEN, through the FEAR network to promote exit from mitosisbecause exit from mitosis brought about by the HOG pathway dependson the FEAR network. Consistent with this idea is our observationthat Cdc5 activity is modestly (2-fold) stimulated by high osmolarity(our unpublished data). Although this twofold increase is notsufficient to bring about exit from mitosis in MEN mutants (ourunpublished data), the increase in Cdc5 activity is likely tocontribute to the rescue of the proliferation defect broughtabout by high osmolarity. Finally, we note that it is of coursealso possible that the HOG pathway stimulates exit from mitosisby a novel yet to be identified pathway that functions in parallelto, both, the FEAR network and the MEN.

An Extracellular Signal Controlling Exit from Mitosis
Several intracellular events, including onset of chromosomesegregation and nuclear position, have been described to regulateexit from mitosis through controlling Cdc14 activity (reviewedin D’Amours and Amon, 2004). High osmolarity is, to ourknowledge, the first extracellular signal shown to affect thiskey phosphatase. Why would high osmolarity promote exit frommitosis? Perhaps stress survival is higher in G₁ than duringmitosis and one function of the HOG pathway could be to pushcells that are delayed in anaphase into G₁ by promoting theactivation of Cdc14 (this study) and stabilization of the CDKinhibitor Sic1 (Escote et al., 2004) to increase their survivalchance.

It is also possible that the HOG pathway is involved in couplingexit from mitosis to events occurring at the bud neck. Previousstudies showed that Sho1 localizes to the bud neck (Raitt etal., 2000; Reiser et al., 2000), a region of the cell whereosmotic stress could occur due to cell wall remodeling and/orcontraction of the acto-myosin ring during cytokinesis. We speculatethat osmotic imbalances in this region signal through the HOGpathway to the mitotic exit machinery to promote exit from mitosis.

Several studies point to a considerable role for MAP kinasepathways in regulating different cell cycle stages in responseto environmental stress (reviewed in Pearce and Humphrey, 2001).Recently, a role for the stress MAP kinase Spc1/Sty1 in mitoticcommitment and recovery from stress has been described in fissionyeast (Petersen and Hagan, 2005) MKK7, an activator of stress-activatedprotein kinase stress-activated protein kinase in mammals, hasbeen shown to couple stress signaling to progression into Mphase and cellular senescence (Wada et al., 2004). Our datanow show that osmotic balance regulates mitotic exit and pointsto a new mechanism in regulation of the final stages of mitosisby stress-activated MAP kinase signaling cascade.

ACKNOWLEDGMENTS

We thank F. Solomon and members of the Amon laboratory for criticalreading of manuscript and for support; and Gustav Ammerer, R.Visintin, and F. Stegmeier for advice and discussions. Thisresearch was supported by a National Institutes of Health GrantGM-56800 to A. A., who is also an investigator of the HowardHughes Medical Institute.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05-11-1067)on April 26, 2006.

* Present address:Merck & Co., One Merck Dr., WhitehouseStation, NJ 07065.

Address correspondence to:Angelika Amon ( angelika{at}mit.edu)

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Albertyn, J., Hohmann, S., Thevelein, J. M., Prior, B. A. (1994). GPD1, which encodes glycerol-3-phosphate dehydrogenase, is essential for growth under osmotic stress in Saccharomyces cerevisiae, and its expression is regulated by the high-osmolarity glycerol response pathway. Mol. Cell. Biol 14, 4135–4144.[Abstract/Free Full Text]

Alepuz, P. M., Jovanovic, A., Reiser, V., Ammerer, G. (2001). Stress-induced MAP kinase Hog1 is part of transcription activation complexes. Mol. Cell 7, 767–777.[CrossRef][Medline]

Alexander, M. R., Tyers, M., Perret, M., Craig, B. M., Fang, K. S., Gustin, M. C. (2001). Regulation of cell cycle progression by Swe1p and Hog1p following hypertonic stress. Mol. Biol. Cell 12, 53–62.[Abstract/Free Full Text]

Bardin, A. J., Boselli, M. G., Amon, A. (2003). Mitotic exit regulation through distinct domains within the protein kinase Cdc15. Mol. Cell Biol 23, 5018–5030.[Abstract/Free Full Text]

Brewster, J. L., de Valoir, T., Dwyer, N. D., Winter, E., Gustin, M. C. (1993). An osmosensing signal transduction pathway in yeast. Science 259, 1760–1763.[Abstract/Free Full Text]

D’Amours, D. and Amon, A. (2004). At the interface between signaling and executing anaphase–Cdc14 and the FEAR network. Genes Dev. 2004 18, 2581–2595.[Abstract/Free Full Text]

de Nadal, E., Casadome, L., Posas, F. (2003). Targeting the MEF2-like transcription factor Smp1 by the stress-activated Hog1 mitogen-activated protein kinase. Mol. Cell Biol 23, 229–237.[Abstract/Free Full Text]

de Nadal, E., Zapater, M., Alepuz, P. M., Sumoy, L., Mas, G., Posas, F. (2004). The MAPK Hog1 recruits Rpd3 histone deacetylase to activate osmoresponsive genes. Nature 427, 370–374.[CrossRef][Medline]

Escote, X., Zapater, M., Clotet, J., Posas, F. (2004). Hog1 mediates cell-cycle arrest in G1 phase by the dual targeting of Sic1. Nat. Cell Biol 6, 997–1002.[CrossRef][Medline]

Grandin, N., de Almeida, A., Charbonneau, M. (1998). The Cdc14 phosphatase is functionally associated with the Dbf2 protein kinase in Saccharomyces cerevisiae. Mol. Gen. Genet 258, 104–116.[CrossRef][Medline]

Hofken, T. and Schiebel, E. (2002). A role for cell polarity proteins in mitotic exit. EMBO J 21, 4851–4862.[CrossRef][Medline]

Hohmann, S. (2002). Osmotic stress signaling and osmoadaptation in yeasts. Microbiol. Mol. Biol. Rev 66, 300–372.[Abstract/Free Full Text]

Jaspersen, S. L., Charles, J. F., Tinker-Kulberg, R. L., Morgan, D. O. (1998). A late mitotic regulatory network controlling cyclin destruction in Saccharomyces cerevisiae. Mol. Biol. Cell 9, 2803–2817.[Abstract/Free Full Text]

Longtine, M. S., McKenzie, A. 3rd, Demarini, D. J., Shah, N. G., Wach, A., Brachat, A., Philippsen, P, Pringle, J. R. (1998). Additional modules for versatile and economical PCR-based gene deletion and modification in Saccharomyces cerevisiae. Yeast 14, 953–961.[CrossRef][Medline]

Maeda, T., Takekawa, M., Saito, H. (1995). Activation of yeast PBS2 MAPKK by MAPKKKs or by binding of an SH3-containing osmosensor. Science 269, 554–558.[Abstract/Free Full Text]

Nanduri, J. and Tartakoff, A. M. (2001). Perturbation of the nucleus: a novel Hog1p-independent, Pkc1p-dependent consequence of hypertonic shock in yeast. Mol. Biol. Cell 12, 1835–1841.[Abstract/Free Full Text]

O’Rourke, S. M. and Herskowitz, I. (2004). Unique and redundant roles for HOG MAPK pathway components as revealed by whole-genome expression analysis. Mol. Biol. Cell 15, 532–542.[Abstract/Free Full Text]

Parkes, V. and Johnston, L. H. (1992). SPO12 and SIT4 suppress mutations in DBF2, which encodes a cell cycle protein kinase that is periodically expressed. Nucleic Acids Res 20, 5617–5623.[Abstract/Free Full Text]

Pearce, A. K. and Humphrey, T. C. (2001). Integrating stress-response and cell-cycle checkpoint pathways. Trends Cell Biol 11, 426–433.[CrossRef][Medline]

Petersen, J. and Hagan, I. M. (2005). Polo kinase links the stress pathway to cell cycle control and tip growth in fission yeast. Nature 435, 507–512.[CrossRef][Medline]

Posas, F. and Saito, H. (1997). Osmotic activation of the HOG MAPK pathway via Ste11p MAPKKK: scaffold role of Pbs2p MAPKK. Science 276, 1702–1705.[Abstract/Free Full Text]

Posas, F. and Saito, H. (1998). Activation of the yeast SSK2 MAP kinase kinase kinase by the SSK1 two-component response regulator. EMBO J 17, 1385–1394.[CrossRef][Medline]

Posas, F., Wurgler-Murphy, S. M., Maeda, T., Witten, E. A., Thai, T. C., Saito, H. (1996). Yeast HOG1 MAP kinase cascade is regulated by a multistep phosphorelay mechanism in the SLN1-YPD1-SSK1 "two-component" osmosensor. Cell 86, 865–875.[CrossRef][Medline]

Proft, M. and Struhl, K. (2002). Hog1 kinase converts the Sko1-Cyc8-Tup1 repressor complex into an activator that recruits SAGA and SWI/SNF in response to osmotic stress. Mol. Cell 9, 1307–1317.[CrossRef][Medline]

Raitt, D. C., Posas, F., Saito, H. (2000). Yeast Cdc42 GTPase and Ste20 PAK-like kinase regulate Sho1-dependent activation of the Hog1 MAPK pathway. EMBO J 19, 4623–4631.[CrossRef][Medline]

Reiser, V., Raitt, D. C., Saito, H. (2003). Yeast osmosensor Sln1 and plant cytokinin receptor Cre1 respond to changes in turgor pressure. J. Cell Biol 161, 1035–1040.[Abstract/Free Full Text]

Reiser, V., Ruis, H., Ammerer, G. (1999). Kinase activity-dependent nuclear export opposes stress-induced nuclear accumulation and retention of Hog1 mitogen-activated protein kinase in the budding yeast Saccharomyces cerevisiae. Mol. Biol. Cell 10, 1147–1161.[Abstract/Free Full Text]

Reiser, V., Salah, S. M., Ammerer, G. (2000). Polarized localization of yeast Pbs2 depends on osmostress, the membrane protein Sho1 and Cdc42. Nat. Cell Biol 2, 620–627.[CrossRef][Medline]

Rep, M., Reiser, V., Gartner, U., Thevelein, J. M., Hohmann, S., Ammerer, G., Ruis, H. (1999). Osmotic stress-induced gene expression in Saccharomyces cerevisiae requires Msn1p and the novel nuclear factor Hot1p. Mol. Cell. Biol 19, 5474–5485.[Abstract/Free Full Text]

Schimmang, T., Tollervey, D., Kern, H., Frank, R., Hurt, E. C. (1989). A yeast nucleolar protein related to mammalian fibrillarin is associated with small nucleolar RNA and is essential for viability. EMBO J 8, 4015–4024.[Medline]

Shou, W., Seol, J. H., Shevchenko, A., Baskerville, C., Moazed, D., Chen, Z. W., Jang, J., Shevchenko, A., Charbonneau, H., Deshaies, R. J. (1999). Exit from mitosis is triggered by Tem1-dependent release of the protein phosphatase Cdc14 from nucleolar RENT complex. Cell 97, 233–244.[CrossRef][Medline]

Stegmeier, F. and Amon, A. (2004). Closing mitosis: the functions of the Cdc14 phosphatase and its regulation. Annu. Rev. Genet 38, 203–232.[CrossRef][Medline]

Stegmeier, F., Visintin, R., Amon, A. (2002). Separase, polo kinase, the kinetochore protein Slk19, and Spo12 function in a network that controls Cdc14 localization during early anaphase. Cell 108, 207–220.[CrossRef][Medline]

Visintin, R. and Amon, A. (2001). Regulation of the mitotic exit protein kinases Cdc15 and Dbf2. Mol. Biol. Cell 12, 2961–2974.[Abstract/Free Full Text]

Visintin, R., Hwang, E. S., Amon, A. (1999). Cfi1 prevents premature exit from mitosis by anchoring Cdc14 phosphatase in the nucleolus. Nature 398, 818–823.[CrossRef][Medline]

Visintin, R., Stegmeier, F., Amon, A. (2003). The role of the polo kinase Cdc5 in controlling Cdc14 localization. Mol. Biol. Cell 14, 4486–4498.[Abstract/Free Full Text]

Wada, T., Joza, N., Cheng, H. Y., Sasaki, T., Kozieradzki, I., Bachmaier, K., Katada, T., Schreiber, M., Wagner, E. F., Nishina, H., Penninger, J. M. (2004). MKK7 couples stress signalling to G2/M cell-cycle progression and cellular senescence. Nat. Cell Biol 6, 215–226.[Medline]

This article has been cited by other articles:

G. Yaakov, A. Duch, M. Garcia-Rubio, J. Clotet, J. Jimenez, A. Aguilera, and F. Posas
The Stress-activated Protein Kinase Hog1 Mediates S Phase Delay in Response to Osmostress
Mol. Biol. Cell, August 1, 2009; 20(15): 3572 - 3582.
[Abstract] [Full Text] [PDF]

D. Melamed, L. Pnueli, and Y. Arava
Yeast translational response to high salinity: Global analysis reveals regulation at multiple levels
RNA, July 1, 2008; 14(7): 1337 - 1351.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

All Versions of this Article:
E05-12-1102v1
17/7/3136 most recent

Alert me when this article is cited

Alert me if a correction is posted

Services

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Google Scholar

Google Scholar

Articles by Reiser, V.

Articles by Amon, A.

Search for Related Content

PubMed

PubMed Citation

Articles by Reiser, V.

Articles by Amon, A.

				D. Melamed, L. Pnueli, and Y. Arava Yeast translational response to high salinity: Global analysis reveals regulation at multiple levels RNA, July 1, 2008; 14(7): 1337 - 1351. [Abstract] [Full Text] [PDF]