Slm1 and Slm2 Are Novel Substrates of the Calcineurin Phosphatase Required for Heat Stress-Induced Endocytosis of the Yeast Uracil Permease

doi:10.1128/MCB.01973-05

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Molecular and Cellular Biology, June 2006, p. 4729-4745, Vol. 26, No. 12
0270-7306/06/$08.00+0 doi:10.1128/MCB.01973-05
Copyright © 2006, American Society for Microbiology. All Rights Reserved.

Slm1 and Slm2 Are Novel Substrates of the Calcineurin Phosphatase Required for Heat Stress-Induced Endocytosis of the Yeast Uracil Permease

Geert Bultynck,¹ Victoria L. Heath,¹^, Alia P. Majeed,¹ Jean-Marc Galan,² Rosine Haguenauer-Tsapis,² and Martha S. Cyert¹^*

Department of Biological Sciences, Stanford University, Stanford, California 94305-5020,¹ Institut Jacques Monod-CNRS, Université Paris VII, 2 place Jussieu, 75005 Paris, France²

Received 9 October 2005/ Returned for modification 14 November 2005/ Accepted 30 March 2006

ABSTRACT

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The Ca²⁺/calmodulin-dependent phosphatase calcineurin promotesyeast survival during environmental stress. We identified Slm1and Slm2 as calcineurin substrates required for sphingolipid-dependentprocesses. Slm1 and Slm2 bind to calcineurin via docking sitesthat are required for their dephosphorylation by calcineurinand are related to the PXIXIT motif identified in NFAT. In vivo,calcineurin mediates prolonged dephosphorylation of Slm1 andSlm2 during heat stress, and this response can be mimicked byexogenous addition of the sphingoid base phytosphingosine. Slmproteins also promote the growth of yeast cells in the presenceof myriocin, an inhibitor of sphingolipid biosynthesis, andregulation of Slm proteins by calcineurin is required for theirfull activity under these conditions. During heat stress, sphingolipidssignal turnover of the uracil permease, Fur4. In cells lackingSlm protein activity, stress-induced endocytosis of Fur4 isblocked, and Fur4 accumulates at the cell surface in a ubiquitinatedform. Furthermore, cells expressing a version of Slm2 that cannotbe dephosphorylated by calcineurin display an increased rateof Fur4 turnover during heat stress. Thus, calcineurin may modulatesphingolipid-dependent events through regulation of Slm1 andSlm2. These findings, in combination with previous work identifyingSlm1 and Slm2 as targets of Mss4/phosphatidylinositol 4,5-bisphosphateand TORC2 signaling, suggest that Slm proteins integrate informationfrom a variety of signaling pathways to coordinate the cellularresponse to heat stress.

INTRODUCTION

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Calcineurin is a Ca²⁺- and calmodulin-regulated serine/threonineprotein phosphatase that is highly conserved from unicellulareukaryotes, such as the budding yeast Saccharomyces cerevisiae,to humans and plays a critical role in Ca²⁺-dependent signalingin these organisms (2). In mammalian cells, calcineurin mediatesa plethora of physiological processes, including T-cell activation,skeletal and cardiac muscle development, long-term potentiation,and neural outgrowth, as well as pathophysiological processessuch as cardiac hypertrophy (7, 11, 28, 34). Specific inhibitorsof calcineurin, FK506 and cyclosporine A, are in wide clinicaluse as immunosuppressants. In yeast cells, calcineurin is dispensablefor growth under standard laboratory conditions. However, calcineurinactivity becomes crucial for survival during specific stressconditions (15). Indeed, calcineurin is activated in mutantswith cell wall defects and by a variety of environmental stresses,including high concentrations of Na⁺, Li⁺, and Mn²⁺ ions; highpH; heat stress; and prolonged exposure to mating factor (reviewedin reference 15). Calcineurin is a heterodimer consisting ofa large catalytic subunit (A subunit; 59 kDa), encoded in S.cerevisiae by two functionally redundant genes, CNA1 and CNA2,and a small regulatory subunit (B subunit; 19 kDa), encodedby CNB1 (16, 17, 48, 53). Extracellular stresses promote a transientrise in the cytosolic Ca²⁺ concentration and subsequent activationof calcineurin through binding of Ca²⁺/calmodulin (reviewedin reference 15). A major role of calcineurin is to regulategene expression via the transcription factor Crz1, which, upondephosphorylation by calcineurin, accumulates in the nucleusand directs the transcription of genes that promote cell survivalduring stress (56, 65, 66, 74).

An important feature of calcineurin signaling is its directinteraction with substrates and regulators via a conserved dockingsite that is distinct from sites of dephosphorylation. Thisproperty was first characterized for NFAT (nuclear factor ofactivated T cells), a family of mammalian transcription factors(1, 55). A small motif with the consensus amino acid sequencePXIXIT is responsible for calcineurin binding to NFAT proteinsand is required for their dephosphorylation (1). Furthermore,this docking site is conserved in other calcineurin-interactingproteins (18, 67). In yeast, calcineurin binds to Crz1 via thePXIXIT-related sequence PIISIQ, and this site is required forits regulation by calcineurin (10).

We searched for novel calcineurin substrates by identifyingcalcineurin-interacting proteins. One of these proteins is Slm2,which was found to interact with the A subunit of calcineurinin a genome-wide yeast two-hybrid screen (69). In this study,we show that Slm2 as well as its homologue, Slm1, binds calcineurinvia a PXIXIT-related motif and that both proteins are dephosphorylatedby calcineurin in vivo and in vitro. In each case, this dephosphorylationrequires the calcineurin-docking site.

Recent studies provide insights into the physiological functionsof Slm1 and Slm2 (4, 27). SLM1 and SLM2 form an essential genepair, and each gene product contains a conserved pleckstrinhomology domain (PH domain) that binds phosphatidylinositol4,5-bisphosphate (PIP₂) (75). The essential lipid kinase Mss4synthesizes PIP₂ in the plasma membrane (19, 40), and this PIP₂production recruits Slm1 and Slm2 to the cell periphery (75).Slm proteins seem to be critical downstream effectors of Mss4/PIP₂,as slm1 ${Delta}$ is synthetically lethal with mss4^ts, and like Mss4,Slm1 and Slm2 are required for polarization of the actin cytoskeleton(4, 27). In addition, Slm1 is phosphorylated by TORC2, a Tor2kinase-containing complex that regulates actin cytoskeletonorganization; this phosphorylation is required for its localizationto the cell periphery (4). Furthermore, an avo3^ts mutant whichlacks an essential subunit of the TORC2 complex is suppressedby SLM1 overexpression (39). Thus, Slm proteins are downstreameffectors of both PIP₂ and TORC2 signaling.

In addition, Slm proteins participate in the cellular responseto heat stress. Heat stress causes a transient increase in PIP₂levels as well as a transient depolarization of the actin cytoskeleton(19). The temporal pattern of Slm1 phosphorylation is modulatedin response to heat stress and parallels the depolarization/repolarizationof the cytoskeleton (4). Furthermore, slm1^ts slm2 ${Delta}$ cells aresuppressed by mutations that activate the cell integrity pathway,a key component of cell tolerance to elevated temperature (4,50). In this study we show that high temperature leads to increasedphosphorylation of Slm1 and Slm2 by protein kinases, which iscounteracted by their dephosphorylation by calcineurin.

Another component of the heat stress response is the productionof sphingolipids. When cells are exposed to high temperature,levels of dihydrosphingosine and phytosphingosine, the majorsphingoid bases in yeast, increase within minutes; these increasedlevels are required for tolerance to heat stress (21, 44). Oneconsequence of phytosphingosine accumulation is inhibition ofnutrient uptake via turnover of permeases, such as the uracilpermease, Fur4 (13, 14, 30). Recently, the PDK1-related kinasesPkh1 and Pkh2 were identified as signaling effectors of phytosphingosine(12, 29, 77). These kinases are required to maintain cell integrityand for endocytosis and act in part through activation of downstreamkinases including Pkc1, Ypk1, and Ypk2 (29, 41, 61). Interestingly,overexpression of YPK1 confers resistance to myriocin, a potentinhibitor of the de novo sphingolipid biosynthesis pathway (68).

Here, we demonstrate a novel role for Slm1 and Slm2 in sphingolipidsignaling and/or metabolism. We show that the Slm proteins arerequired for growth of yeast cells in the presence of myriocinand for endocytosis of Fur4 during heat stress. Both of theseaspects of Slm function are altered by mutations that abrogatethe ability of calcineurin to dephosphorylate Slms, suggestingthat calcineurin acts through Slm1 and Slm2 to regulate sphingolipid-dependentevents. Thus, Slm1 and Slm2 apparently coordinate TORC2, Mss4/PIP₂,sphingolipid, and Ca²⁺/calcineurin signaling to drive actinpolarization and promote endocytosis of a nutrient permeaseduring heat stress.

MATERIALS AND METHODS

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Yeast strains and media. Yeast media and culture conditions were essentially as previouslydescribed (62), except that twice the levels of amino acidsand nucleotides were used in synthetic media. Yeast transformationswere performed with the lithium acetate method (5). Yeast strainsare listed in Table 1; strains from the yeast deletion collectionwere purchased from Open Biosystems (Huntsville, AL).

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TABLE 1. Yeast strains used in this study

VHY61 is a haploid segregant of BY4743, slm2 ${Delta}$ ::KAN^R (deletioncollection). To create GBY59, the SLM1 open reading frame (ORF)of VHY61 transformed with pRS316-SLM2 was replaced by the natMX4cassette via PCR, using pAG25 as the template (32). This strainwas then transformed with all other Slm alleles expressed fromdifferent plasmids. The pRS316-Slm2 plasmid was lost by streakingout the transformants on selective medium supplemented with5-fluorootic acid (5FOA; U.S. Biochemicals, Swampscott, MA).

The plasmids used in this study are reported in Table 2. RecombinantDNA procedures were performed as previously described (5). Allgenes were initially cloned by amplification of genomic DNAwith Vent polymerase or with Taq high-fidelity polymerase (Invitrogen,Beverly, MA) to create fragments flanked by restriction sites.Cloned genes were subcloned in different expression vectorsby PCR amplification of plasmid DNA with PfuUltra HotStart polymerase(Stratagene, Cedar Creek, TX). All clones were sequenced bySequetech Corporation (Mountain View, CA).

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TABLE 2. Plasmids used in this study

For yeast two-hybrid studies, the pGBT9 and pACT2 vectors wereused to create GAL4-binding and GAL4 activation domain fusions,respectively. All full-size and truncated versions of SLM1 andSLM2 were cloned as NcoI/XhoI fragments into pACT2 and as XmaI/SalIfragments into pGBT9. A PCR-based deletion strategy was usedto delete codons 639 to 644 of SLM2, encoding PEFYIE, and codons672 to 677 of SLM1, encoding PNIYIQ. All glutathione S-transferase(GST) and green fluorescent protein (GFP) expression plasmidswere constructed by cloning SLM1 and SLM2 as XmaI/XhoI fragments.For pRS316 and pRS313 plasmids, we first cloned the promotersof SLM1 and SLM2 (500-bp sequences upstream of the respectiveORFs) as SpeI/XmaI fragments. We then cloned the different SLMalleles as XmaI/XhoI fragments. FUR4 was subcloned in the pVT102-Uoverexpression plasmid as an XbaI/XhoI fragment amplified byPCR, using pfF as the template (70).

Chemical compounds. Myriocin (Sigma, St. Louis, MO) was dissolved in methanol ata stock concentration of 1 mg/ml and was stored at 4°C.Aureobasidin A (Takara Mirus Bio, Madison, WI) was dissolvedin ethanol at a stock concentration of 1 mg/ml and was storedat 4°C. Phytosphingosine (Sigma) was dissolved in ethanolat a stock concentration of 20 mM and was stored at –20°C.All these stock solutions were put at room temperature 30 minprior to their addition to media. FK506 (LC Laboratories, Woburn,MA) was dissolved in a mixture of 90% ethanol and 10% Tween20 at a stock concentration of 20 mg/ml and stored at 4°C.FK506 was used at a final concentration of 2 µg/ml.

Spot assays. Growth of various strains was assessed by spotting serial dilutionsof stationary-phase yeast cultures on yeast-peptone-dextrose(YPD) plates containing various drugs or selective medium (foryeast two-hybrid analysis). Cultures were diluted to an opticaldensity at 600 nm (OD₆₀₀) of 2.0, and five or six fivefold serialdilutions were prepared and transferred to the plates. Plateswere incubated at 30°C for 2 to 3 days unless otherwiseindicated.

Yeast two-hybrid analysis. Yeast two-hybrid assays were performed by introducing combinationsof Gal4p activation and binding domain fusions into strain PJ69-4A,which contains a GAL1 promoter-HIS3 reporter gene, a GAL2 promoter-ADE2reporter gene, and a GAL7 promoter-lacZ reporter gene (42, 43).Strains were grown in selective medium and spotted onto syntheticmedium containing and lacking either histidine or adenine. ß-Galactosidaseactivity was determined in exponentially growing yeast cellsat 30°C as follows. Cells were harvested and washed onceand the cell pellets were frozen. Cells were broken using glassbead lysis in breaking buffer (100 mM Tris [pH 8], 20% glycerol,1 mM dithiothreitol [DTT]) plus protease inhibitors (1 mM phenylmethylsulfonylfluoride [PMSF], 1 mM benzamidine, 2 µg/ml leupeptin,2 µg/ml aprotinin). ß-Galactosidase activitywas measured at 30°C in a microtiter plate using 10 µlof total protein extract, 90 µl of Z-buffer (100 mM Na₂HPO₄,40 mM NaH₂PO₄, 10 mM KCl, 1 mM MgSO₄, 0.027% ß-mercaptoethanol),and 20 µl of 4 mg/ml ONPG (O-nitrophenyl-ß-D-galactopyranoside;Sigma). Protein concentrations of all cell extracts were determinedusing a Bio-Rad protein assay (Bio-Rad, Richmond, CA) and wereused to calculate the specific ß-galactosidase activity.Values result from averages of two independent extracts, eachmeasured in triplicate.

Isolation of GST-tagged proteins. Yeast cells expressing GST-Slm1 or GST-Slm2 were grown at 30°Cin synthetic medium lacking uracil with 4% raffinose as thecarbon source. Cells were diluted to an OD₆₀₀ of 0.2 in syntheticmedium lacking uracil with 4% raffinose as the carbon source.After 4 h, expression of the GST fusion proteins was inducedby the addition of 2% galactose for 4 h. When indicated in Fig.2, 3, and 5, FK506 (2 µg/ml) was added 30 min prior tothe addition of galactose. Cells were harvested by centrifugation,and cell pellets were frozen at –80°C prior to thepreparation of extracts. Cells were broken by using glass beadlysis in modified radioimmunoprecipitation assay buffer (20mM Tris-HCl [pH 7.4], 2 mM EDTA, 750 mM NaCl, 1% Triton X-100,1 mM DTT), supplemented with protease inhibitors (1 mM PMSF,1 mM benzamidine, 1 µg/ml pepstatin A, 1 µg/ml leupeptin,1 µg/ml aprotinin) and phosphatase inhibitors (5 mM sodiumphosphate, 10 mM sodium molybdate, 20 mM sodium fluoride, 10mM sodium pyrophosphate, 5 mM EGTA, and 5 mM EDTA). Proteinconcentrations of all cell extracts were determined using aBio-Rad protein assay. Protein extracts (150 to 350 µg)were diluted fivefold in dilution buffer (20 mM Tris-HCl [pH7.4], 2 mM EDTA, 150 mM NaCl, 1 mM DTT, 1 mM PMSF, 1 mM benzamidine,1 µg/ml pepstatin A, 1 µg/ml leupeptin, 1 µg/mlaprotinin) and incubated for 2 h with glutathione-Sepharosebeads preequilibrated with dilution buffer at 4°C. Beadswere washed three times in wash buffer (20 mM Tris-HCl [pH 7.4],2 mM EDTA, 150 mM NaCl, 0.5% Triton X-100, 1 mM DTT, 1 mM PMSF,1 mM benzamidine, 1 µg/ml pepstatin A, 1 µg/ml leupeptin,1 µg/ml aprotinin). GST fusion proteins were eluted insodium dodecyl sulfate (SDS) sample buffer, separated on a 6.75%SDS-polyacrylamide gel electrophoresis (PAGE) gel, and transferredto a nitrocellulose membrane. Blots were incubated either withthe rabbit polyclonal antiphosphorylated proteins (Pan) antibody(diluted 1/250; Zymed Laboratories Inc., South San Francisco,CA) or with the mouse 4C10 monoclonal anti-GST (diluted 1/1,000;Covance/Berkeley Antibody Co., Richmond, CA) and then with horseradishperoxidase-conjugated anti-rabbit or anti-mouse immunoglobulin(Amersham, Arlington Heights, IL).

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FIG. 2. Calcineurin interacts with Slm1 and Slm2 via a C-terminal PXIXIT-related motif. (A) Mapping of the calcineurin-docking site on Slm1 and Slm2 via yeast two-hybrid assays. The PJ69-4A strain containing the GAL4 DNA-binding domain fusion of CNA1 (DBD) was transformed with different truncations or internal deletions of SLM1 and SLM2. Positive interactions were identified as growth on synthetic medium lacking histidine (3 days at 30°C). GAL4 activation domain fusions (AD) that interacted with Cna1 are indicated as "+", and those that did not interact are indicated as "–." (B) Relevant parts of the amino acid sequences of Slm2 and Slm1 with the conserved calcineurin-docking sites, PXIXIT-related motifs, underlined. (C) Deletion of the calcineurin-docking site abolishes the calcineurin-dependent dephosphorylation of Slm1 and Slm2. Wild-type GST-SLM2 (GBY115) and GST-SLM1 (GBY117) and their counterparts lacking the calcineurin-docking site, GST-SLM2^PEFYIE (GBY116) and GST-SLM1^PNIYIQ (GBY118), were expressed in a strain deleted for slm1 ${Delta}$ and slm2 ${Delta}$ . Cells were grown in selective synthetic medium supplemented with 4% raffinose. One culture was treated with FK506 (as indicated). GST fusion proteins were purified from cell extracts, subjected to SDS-PAGE, and Western blotted with anti-phospho and anti-GST antibodies. (D) Deletion of the calcineurin-docking site in SLM1 or SLM2 does not impair growth. An slm1 ${Delta}$ slm2 ${Delta}$ strain expressing SLM2 under the control of its own promoter on a pRS316 plasmid (GBY059) was transformed with either pRS313 (vector; GBY152), pRS313-SLM2 (Slm2; GBY153), pRS313-SLM2^PEFYIE (Slm2^PEFYIE; GBY154), pRS313-SLM1 (Slm1; GBY155), or pRS313-SLM1^PNIYIQ (Slm1^PNIYIQ; GBY156). Serial dilutions of saturated cell cultures were plated on synthetic medium lacking uracil and histidine (-ura-his) and on synthetic medium lacking histidine but supplemented with 5FOA (-his+5-FOA). Cells were grown for 3 days at 30°C. (E) Localization of Slm proteins and actin cytoskeleton stabilization by Slm proteins are not dependent on the calcineurin-docking site. slm1 ${Delta}$ slm2 ${Delta}$ cells expressing GFP-SLM2 (GBY104), GFP-SLM2^PEFYIE (GBY105), GFP-SLM1 (GBY106), or GFP-SLM1^PNIYIQ (GBY107) were grown to log phase and visualized by differential interference microscopy (DIC) and by fluorescence microscopy (GFP). Actin cytoskeleton was visualized with Texas Red-X phalloidin in formaldehyde-fixed cells.

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FIG. 3. Phosphorylation of Slm1 and Slm2 is increased during heat stress when their calcineurin-dependent dephosphorylation is compromised. (A) GST-SLM2 (GBY115) and GST-SLM2^PEFYIE (GBY116) were expressed in a strain lacking slm1 and slm2. Cells were grown at 25°C in selective synthetic medium and expression was induced with 2% galactose. One culture was treated with FK506 (2 µg/ml) as indicated. Cells were shifted to 37°C and samples were taken at indicated time points (t). GST fusion proteins were purified from cell extracts and subjected to SDS-PAGE and Western blotting with anti-phospho and anti-GST antibodies. Immunoreactive bands were quantified using ImageJ software. The ratio of the anti-phospho signal over the anti-GST signal was plotted in arbitrary units (A.U.) as a function of time. (B) An approach similar to that described for panel A was taken for GST-SLM1 (GBY117) and GST-SLM1^PNIYIQ (GBY118).

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FIG. 5. The heat stress-induced increase in Slm1 and Slm2 phosphorylation is independent of Tor2p. Overnight cultures of wild-type (wt; JK9-3da) and tor2^ts (SH121) cells expressing either GST-Slm2 or GST-Slm1 were diluted to an OD₆₀₀ of 0.2 and grown at 25°C for 4 h. To one set of cultures, FK506 (final concentration, 2 µg/ml) or solvent (90% ethanol/10% Tween 20) was added and cells were shifted to 38°C. After 30 min, galactose (2%) was added to induce protein expression and cells were grown for another 4 h at 38°C. GST fusion proteins were purified from cell extracts and subjected to SDS-PAGE and Western blotting with anti-phospho and anti-GST antibodies.

Detection and quantification of immunoreactive bands by immunoblotting. Immunoreactive bands on Western blots were visualized with anECL kit (Pierce, Rockford, IL) and subsequent exposure to BiomaxMR film (VWR, San Francisco, CA). For each blot, multiple exposures,ranging from 6 seconds to several minutes, were taken. Eachexposure was scanned to obtain a digital image, and immunoreactivebands were quantified using ImageJ (version 1.34n) software(http://rsb.info.nih.gov/ij/). Data presented in the figuresrepresent analysis of a single optimal exposure for each blot.This optimal exposure was determined empirically; an exposurefor which the signal from the most intense band was $≤$ 30% of itsobserved maximum was used, thus ensuring that quantificationwas not distorted by signal saturation. In each case, from twoto four independent experiments were conducted; the data displayedin the figures depict results from a single representative experiment.

In vitro phosphatase assay. DD12 cells expressing GST-Slm1 or GST-Slm2 were grown for 4h in synthetic medium lacking uracil and methionine with 4%raffinose as the carbon source. Expression of the GST fusionproteins was induced by the addition of 2% galactose. Lysisof the cells and purification of the GST fusion proteins wereperformed as described above. GST fusion proteins bound to theglutathione-Sepharose 4B beads were washed twice in wash buffercontaining protease inhibitors and phosphatase inhibitors, twicein wash buffer containing protease inhibitors only, and twicein CP buffer (50 mM Tris-HCl [pH 7.5], 1 mM MgCl₂, 1 mM DTT)containing protease inhibitors. Washed beads were divided amongfour tubes prior to the administration of different phosphatasetreatments. Phosphatase assays were performed in a total of100 µl in CP buffer for calcineurin and in the suppliedbuffer for ${lambda}$ -phosphatase (New England Biolabs, Beverly, MA);500 U of recombinant human calcineurin (Calbiochem, San Diego,CA), 2,600 U of calmodulin (Calbiochem), or 10 µl of ${lambda}$ -phosphatase(New England Biolabs) was used per assay. Where indicated, CaCl₂was added to a final concentration of 40 mM and EGTA to 10 mM.Phosphatase assays were incubated at 30°C for 30 min; thesupernatant was then removed, and SDS-PAGE sample buffer wasadded to the beads. Samples were analyzed by SDS-PAGE (7.5%gels) and blotted as described above. Immunoreactive bands werevisualized as described above.

Fluorescence microscopy. The localization of GFP-Slm2, GFP-Slm2^PEFYIE, GFP-Slm1, andGFP-Slm1^PNIYIQ was examined in strains GBY104 through GBY107.Liquid cultures were set up in synthetic medium lacking histidineand supplemented with methionine (75 mg/liter). Log-phase cultures(OD₆₀₀, 1.0) were concentrated by brief centrifugation and mountedon microscope slides. Cells expressing a single GFP fusion werevisualized with a Nikon Eclipse E600 microscope with fluorescenceoptics and an HB100 mercury lamp. Fluorescein filter sets (ChromaTechnology Co., Brattleboro, VT) were used to visualize GFP.Photos were taken with a Hamamatsu 47420-95 digital charge-coupled-devicecamera and QED software (QED Imaging). Actin cytoskeleton stainingwas performed on cells grown to log phase. Cells were then fixedfor 30 min at room temperature by the direct addition of 37%formaldehyde stock to a final concentration of 5%. Fixed cellswere collected and washed twice with phosphate-buffered salinesupplemented with 1 mg/ml bovine serum albumin. Then, 0.04 U/µlof Texas Red-X phalloidin (Molecular Probes, Eugene, OR) wasadded for 30 min at room temperature to stain actin. Cells werewashed three times with phosphate-buffered saline supplementedwith 1 mg/ml bovine serum albumin. Cells were resuspended inmounting medium and visualized as described above, except thata rhodamine filter was used. Only those cells in which the budwas significantly smaller than the mother cell were analyzed.

Fur4 turnover. Wild-type cells and slm1^ts slm2 ${Delta}$ cells transformed with pVT102u-Fur4(pGB047) were grown at 25°C in selective synthetic mediumlacking uracil to log phase. Cells were shifted to 40°Cafter OD₆₀₀ was measured, and at the indicated time points,3 OD₆₀₀ units of yeast cells (i.e., 3 ml of culture at an OD₆₀₀of 1.0 or the equivalent) was removed. Cells were harvestedand resuspended in H₂O, yielding a total volume of 500 µl.Cells were lysed for 10 min on ice by adding 50 µl 1.85M NaOH supplemented with 300 mM ß-mercaptoethanol.Proteins were precipitated on ice for 10 min by adding 50 µlof 50% trichloroacetic acid. Proteins were collected by centrifugationand the protein pellets were dissolved in 120 µl urea-SDSsample buffer (8 M urea, 5% SDS, 200 mM Tris-HCl [pH 6.8], 0.1mM EDTA [pH 8], 0.1% bromophenol blue, 100 mM DTT) supplementedwith 100 mM Tris. Samples were heated for 10 min at 37°Cjust before being loaded onto a 4 to 15% SDS-PAGE gel (Bio-Rad,Richmond, CA). After Western blotting to nitrocellulose, membraneswere incubated with the rabbit polyclonal anti-Fur4 (1/15,000dilution) and with the mouse monoclonal 22C5 anti-Pgk1p (1/5,500dilution; Molecular Probes). After image analysis, the anti-Fur4signal was corrected for the Pgk1p loading control, and allvalues were normalized to the 0-min time point. A similar approachwas taken for determining the Fur4 turnover rate in cells expressingGST-Slm2, GST-Slm2^PEFYIE, GST-Slm1, or GST-Slm1^PNIYIQ, exceptthat pfF was used for the overexpression of Fur4.

Uracil uptake assay. Exponentially growing wild-type or slm1^ts slm2 ${Delta}$ cells transformedwith pVT102u-Fur4 (pGB047) and grown in selective syntheticmedium lacking uracil at 25°C were preshifted 10 min at40°C. At time zero, cells were treated with cycloheximide(10 µg/ml). The uracil uptake was measured as previouslydescribed (31). Yeast cultures (1 ml) were incubated with 5µM [¹⁴C]uracil (Amersham, Arlington Heights, IL) for 20s at 30°C and quickly filtered through Whatman GF/C filters.Filters were washed twice with ice-cold water and assessed forradioactivity.

Membrane preparation for detection of ubiquitinated Fur4. Exponentially growing yeast cells transformed with pVT102u-Fur4(pGB047) and grown in selective synthetic medium lacking uracilat 25°C were shifted to 40°C. Ten minutes after heatshock, cycloheximide (100 µg/ml) was added for 50 min.Yeast cells (8.5 OD₆₀₀ units) were harvested before (0 min)and after (60 min) the temperature shift by centrifugation inthe presence of 10 mM sodium azide, washed once in distilledwater plus 10 mM sodium azide, and used to prepare membrane-enrichedfractions, as described in reference 23. Washed cells were transferredto a conical 1.5-ml Eppendorf tube and suspended in 150 µlof lysis buffer (100 mM Tris-HCl [pH 7.4], 150 mM NaCl, and5 mM EDTA plus protease inhibitors and 25 mM freshly preparedN-ethylmaleimide to prevent artifactual deubiquitination). Allsubsequent steps were carried out at 4°C. Chilled glassbeads (150 µl) were added, and the cells were lysed byvigorous vortex mixing seven times for 1 min each, separatedby 1-min intervals. The homogenate was collected and centrifugedat 3,000 rpm for 2 min to remove unbroken cells and debris.The total protein extract was centrifuged for 45 min at 16,100x g. This pellet was washed by suspension in 100 ml lysis buffersupplemented with 5 M urea, incubated for 30 min on ice, andcentrifuged for 45 min at 16,100 x g. The resulting pellet wassuspended in 100 µl of lysis buffer, and trichloroaceticacid was added to 10% to precipitate proteins and to preventproteolysis by residual endogenous proteases. Protein precipitateswere collected by sedimentation (16,100 x g, 45 min). The proteinprecipitates were suspended in 40 µl urea-SDS sample buffersupplemented with 100 mM Tris, and 8 µl of this mixturewas analyzed on a 4 to 15% SDS-PAGE gel (Bio-Rad, Richmond,CA). After the Western blotting procedure, membranes were incubatedwith anti-Fur4, developed, stripped with Restore Western blotstripping solution (Pierce, Rockford, IL), and reprobed withanti-ubiquitin (P4D1 monoclonal; Santa Cruz Biotechnology, SantaCruz, CA).

RESULTS

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Slm1 and Slm2 interact with and are physiological substrates of calcineurin. Genome-wide yeast two-hybrid analyses demonstrated an interactionbetween the A subunit of calcineurin and the ORF YNL047C, characterizedas SLM2. We used yeast two-hybrid assays to confirm this observationand to investigate whether the A subunit of calcineurin wasalso able to interact with Slm1, which is 53% identical to Slm2at the protein level. Cna1 and Cna2 were fused in frame withthe Gal4 DNA-binding domain, whereas Slm1 and Slm2 were fusedin frame with the Gal4 activation domain. Combinations of theseconstructs were expressed in strain PJ69-4A, which containsthree different reporter genes, each driven by a different promoter.The GAL1 promoter-HIS3 reporter is activated by low- and high-affinityinteractions, whereas the more stringent GAL2 promoter-ADE2reporter and GAL7 promoter-lacZ reporter are activated onlyby high-affinity interactions. As indicated in Fig. 1A, bothSlm1 and Slm2 interacted with Cna1 as well as Cna2 and allowedgrowth of strains on medium lacking histidine. However, onlySlm2 was able to activate the ADE2 and lacZ reporter genes,suggesting that Slm2 interacts with Cna1 and Cna2 with an affinityhigher than that of Slm1. We believe these differences in reporteractivation reflect differences in affinity, since the Slm1-and Slm2-Gal4 activation domain fusion proteins are expressedat similar levels and show identical interactions in two-hybridassays with other gene products, such as Avo2, a subunit ofthe TORC2 protein kinase complex (data not shown).

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FIG. 1. Slm1 and Slm2 interact with and are dephosphorylated by calcineurin. (A) Slm1 and Slm2 interact with Cna1 and Cna2 in yeast two-hybrid assays. A strain (PJ69-4A) containing GAL1-HIS3, GAL2-ADE2, and GAL7-lacZ reporter genes was transformed with combinations of GAL4 DNA-binding domain fusions of CNA1 and CNA2 (DBD) and GAL4 activation domain fusions of SLM1 and SLM2 (AD), as indicated. Serial dilutions of saturated cultures were plated on synthetic medium containing histidine and adenine (+his+ade) or lacking histidine (-his) or adenine (-ade), and incubated for 3 days at 30°C. ß-Galactosidase (ßgal) activity in the different strains was measured in liquid cultures as described in Materials and Methods and reported as units/µg of protein. (B) Slm1 and Slm2 are both dephosphorylated in vivo by calcineurin. Wild-type cells (wt; YPH499) and cells lacking the B subunit of calcineurin (cnb1 ${Delta}$ ; DD12) expressing GST-SLM2 (GBY030 and GBY032) or GST-SLM1 (GBY031 and GBY033) were grown to log phase. GST fusion proteins were purified from extracts, subjected to SDS-PAGE, and Western blotted with anti-phospho or anti-GST antibody. (C) Slm1 and Slm2 are both dephosphorylated in vitro by calcineurin. GST-Slm1 (GBY032) and GST-Slm2 (GBY033) purified from cnb1 ${Delta}$ cells were treated with recombinant calcineurin, calmodulin (CaM), CaCl₂, EGTA, or ${lambda}$ -phosphatase as indicated in the left-hand lanes (see Materials and Methods). These samples, together with untreated GST-Slm1 and GST-Slm2 purified from cnb1 ${Delta}$ cells, were then subjected to SDS-PAGE and Western blotted with anti-phospho and anti-GST antibodies.

Since Slm1 and Slm2 interacted with both calcineurin A subunits,we determined whether they were substrates of calcineurin invivo (Fig. 1B). Functional N-terminal GST fusions of Slm1 andSlm2 were expressed in wild-type and calcineurin-null cells(cnb1 ${Delta}$ , lacking the calcineurin regulatory B subunit). Afterpurification of GST-Slm1 and GST-Slm2 on glutathione-Sepharose4B beads, we examined their electrophoretic mobilities by Westernblotting with anti-GST antibodies. In addition, we determinedthe extents of phosphorylation of Slm1 and Slm2 by Western blottingwith a mixture of antibodies that recognizes phosphorylatedserine, threonine, and tyrosine residues (see Materials andMethods). We will refer to this as the phospho-antibody. Asshown in Fig. 1B, Slm2 displayed a calcineurin-dependent changein phosphorylation, as is evident from the shift in electrophoreticmobility (anti-GST blot) and from the dramatic difference inthe extents of phosphorylation (anti-phospho blot) in extractsof wild-type cells versus cnb1 ${Delta}$ cells. Slm1 also showed calcineurin-dependentchanges in electrophoretic mobility and in the extent of phosphorylation;however, the differences were more subtle. Quantification ofthe signal obtained with the phospho-antibody showed an $~$ 20 to30% increase in the phosphorylation of GST-Slm1 in cells lackingcalcineurin activity that was consistently and reproduciblyobserved. As we will show (see Fig. 3), the dephosphorylationof Slm1 by calcineurin becomes more evident under specific stressconditions (such as heat stress), leading to hyperphosphorylationof GST-Slm1 when calcineurin function is compromised. Thesedata indicate that both Slm1 and Slm2 display calcineurin-dependentchanges in phosphorylation in vivo.

We then used an in vitro dephosphorylation assay to show thatSlm1 and Slm2 are direct substrates of calcineurin. GST-Slm1and GST-Slm2, purified from calcineurin-deficient cells, showedincreased mobilities and reduced extents of phosphorylationwhen incubated with purified Ca²⁺/CaM-activated calcineurin(Fig. 1C). These changes were abolished by inhibiting calcineurinwith EGTA, a Ca²⁺ chelator (Fig. 1C). Calcineurin was able toperform a robust dephosphorylation of GST-Slm2 (>80% reductionin phosphorylation in comparison to untreated GST-Slm2) andhad a partial effect on the phosphorylation state of GST-Slm1( $~$ 30% reduction in phosphorylation in comparison to untreatedGST-Slm1). In agreement with these changes in the extent ofphosphorylation, the protein samples incubated with active purifiedcalcineurin showed increased electrophoretic mobility (anti-GSTblot). As a control, both proteins were completely dephosphorylatedby ${lambda}$ -phosphatase treatment.

Hence, both Slm1 and Slm2 are calcineurin substrates. However,both the in vivo and in vitro experiments show that while themajority of Slm2 phosphorylation is subject to dephosphorylationby calcineurin, only some of the phosphorylated sites of Slm1are dephosphorylated by calcineurin.

Calcineurin binds to a conserved C-terminal PXIXIT-related motif in Slm1 and Slm2. To further examine the physiological relevance of the calcineurin-dependentdephosphorylation of Slm1 and Slm2, we mapped the calcineurin-bindingsite in Slm1 and Slm2. A series of N-terminal deletion constructsof Slm1 and Slm2 was tested for interaction with Cna1 by useof the yeast two-hybrid method (Fig. 2A). All N-terminally truncatedproteins interacted with calcineurin, suggesting that the calcineurin-dockingsite was located in the C-terminal protein of Slm1 and Slm2.Many proteins interact with calcineurin via a docking motifwith a consensus PXIXIT sequence. We found a potential PXIXIT-relatedmotif in the C-terminal tail of Slm2 (PEFYIE) that had a similarcounterpart in Slm1 (PNIYIQ) (Fig. 2B). Slm1 and Slm2 lackingtheir C-terminal tails (amino acids [aa] 1 to 672 and aa 1 to639, respectively) failed to interact with Cna1, as did mutantconstructs in which only the PXIXIT motifs were deleted (Slm1,aa 1 to 686^PNIYIQ, and Slm2, aa 1 to 657^PEFYIE) (Fig. 2A). Similarresults were obtained for interactions with Cna2 (data not shown).In contrast, deletion of the PXIXIT motif had no effect on Slm1or Slm2 interaction with Avo2, as measured by use of the two-hybridtechnique (data not shown). Thus, for both Slm1 and Slm2, wedefined a small PXIXIT-related motif required specifically fortheir interaction with calcineurin.

For other substrates, eliminating the calcineurin-docking siteabolishes their calcineurin-dependent dephosphorylation. Hence,we investigated the effect of deleting the PXIXIT motif in Slm1and Slm2. We expressed Slm1^PNIYIQ and Slm2^PEFYIE as GST fusionproteins in cells lacking endogenous Slm1 and Slm2 (Fig. 2C).In contrast to what was seen for the wild-type GST-Slm2 andGST-Slm1, GST-Slm2^PEFYIE and GST-Slm1^PNIYIQ showed no differencein electrophoretic mobilities or extents of phosphorylationin extracts of cells containing or lacking calcineurin. Furthermore,it was evident that in contrast to GST-Slm2, GST-Slm2^PEFYIEaccumulated in the phosphorylated form even in cells containingcalcineurin. We observed a similar behavior for GST-Slm1^PNIYIQ;however, the differences were less striking due to the partialeffects of calcineurin on Slm1 dephosphorylation. We concludefrom these findings that calcineurin binding to Slm1 and Slm2via their PXIXIT motifs is required for calcineurin-dependentdephosphorylation of these proteins and that GST-Slm1^PNIYIQand GST-Slm2^PEFYIE are hyperphosphorylated in vivo.

Next, we tested whether the PXIXIT-related motif was requiredfor Slm protein function or localization. SLM1 and SLM2 areredundant for an essential function (4). Therefore, to testthe abilities of different SLM alleles to support growth, weintroduced them into an slm1 ${Delta}$ slm2 ${Delta}$ strain that also containeda URA3 CEN plasmid expressing SLM2 from its own promoter (pGB013).We then tested whether the different strains could grow in theabsence of pGB013 (i.e., on plates containing 5FOA) (Fig. 2D).As expected, cells expressing the vector alone were not ableto grow, confirming that SLM1 and SLM2 form an essential genepair. Wild-type SLM1 and SLM2 as well as their PXIXIT-deletedcounterparts were able to promote growth with similar levelsof efficiency. This shows that calcineurin-dependent regulationof Slm1 and Slm2 is dispensable for growth under standard conditions.Calcineurin is essential for yeast growth under certain stressconditions, including ionic stress (Na⁺, Li⁺, Mn²⁺, Ca²⁺), highpH, and the presence of cell wall-disrupting compounds (calcofluorwhite and Congo red). However, no growth defects were observedfor the strains expressing PXIXIT-deleted products of SLM1 andSLM2 alleles under any of these stress conditions (data notshown). Slm1 and Slm2 localize to punctate patches at the cellsurface (4, 27), and GFP-Slm proteins lacking the PXIXIT motifdisplayed an identical localization (Fig. 2E). In addition,Slm1 and Slm2 are required for polarization of the actin cytoskeleton.We used Texas Red-phalloidin to visualize cellular actin inbudded yeast cells and observed no differences in actin cytoskeletonorganization between cells expressing either wild-type Slm1or Slm2 or the corresponding mutant proteins lacking the calcineurin-dockingsite (Fig. 2E).

Thus, calcineurin-dependent regulation of Slm1 and Slm2 is notrequired for their abilities to support growth, to localizeto the cell periphery, or to polarize the actin cytoskeleton.

Slm1 and Slm2 are dephosphorylated by calcineurin during heat stress and after addition of sphingolipids. During heat stress, Slm1 is transiently dephosphorylated andsubsequently rephosphorylated (4). Hence, we tested the effectof calcineurin on Slm protein phosphorylation under these conditions.We expressed Slm1 and Slm2 and their PXIXIT-deleted counterparts,Slm1^PNIYIQ and Slm2^PEFYIE, as GST fusion proteins in the strainlacking endogenous Slm1 and Slm2 (Fig. 3). Shifting cells from25°C to 37°C induced no detectable change in the phosphorylationof GST-Slm2 and resulted in a slight increase in the net phosphorylationof GST-Slm1 after 75 min (20% increase). However, the effectof heat stress on phosphorylation of GST-Slm1 and GST-Slm2 becamemuch more apparent when calcineurin activity was inhibited withthe specific inhibitor FK506 or when the calcineurin-dockingsite of GST-Slm1 or that of GST-Slm2 was deleted. After we shiftedthe temperature from 25°C to 37°C, we found a time-dependentincrease in the phosphorylation of GST-Slm2 purified from cellstreated with FK506 and of purified GST-Slm2^PEFYIE ( $~$ 10-fold increasein both cases) (Fig. 3A). Phosphorylation of GST-SLM1 purifiedfrom cells treated with FK506 and of purified GST-Slm1^PNIYIQalso increased after a shift to high temperature, although themagnitude of the change was smaller (approximately two- to threefold)(Fig. 3B).

Heat stress transiently increases biosynthesis of sphingoidbases (phytosphingosine and dihydrosphingosine), which in turnactivate downstream kinases (21, 44). Therefore, we tested whetherthe addition of phytosphingosine could mimic the effect of elevatedtemperature to promote phosphorylation of GST-Slm1^PNIYIQ andGST-Slm2^PEFYIE (Fig. 4). Indeed, as observed for heat stress(Fig. 3), the addition of 20 µM phytosphingosine to cellsat 25°C increased the phosphorylation of GST-Slm2^PEFYIE( $~$ 10-fold increase) (Fig. 4A) and that of GST-Slm1^PNIYIQ ( $~$ 2-foldincrease) (Fig. 4B). Together, these results indicate that throughincreased synthesis of phytosphingosine, heat stress triggersan increase in Slm1 and Slm2 phosphorylation that is largelycounteracted in vivo by calcineurin-mediated dephosphorylation.

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FIG. 4. Phytosphingosine mimics the heat stress-induced phosphorylation of Slm1 and Slm2. GST-SLM2 (GBY115), GST-SLM2^PEFYIE (GBY116), GST-SLM1 (GBY117), and GST-SLM1^PNIYIQ (GBY118) were expressed in a strain lacking slm1 and slm2. Cells were grown at 25°C in selective synthetic medium and expression was induced with 2% galactose. Samples were taken just before the addition of 20 µM phytosphingosine (0 min) and at time points (t) 45, 90, and 120 min after the addition of phytosphingosine. GST fusion proteins were purified from cell extracts and subjected to SDS-PAGE and Western blotting with anti-phospho and anti-GST antibodies. Immunoreactive bands were quantified as described in Materials and Methods. The ratio of the anti-phospho signal over the anti-GST signal was plotted in arbitrary units (A.U.).

These data suggest that both elevated temperature and additionof phytosphingosine lead to activation of calcineurin in vivoand consequently to increased Slm protein dephosphorylation.We therefore tested the effects of heat stress and phytosphingosineon calcineurin by monitoring the activity of Crz1, a calcineurin-regulatedtranscription factor. We measured expression of a 4x CDRE::lacZreporter gene which is specifically activated by Crz1 (65).Table 3 shows that elevated temperature as well as the additionof phytosphingosine (20 µM) increased Crz1 activity andthat this increased activity was completely inhibited by FK506.Thus, the increase in Crz1 activity reflects activation of calcineurinin response to heat stress or incubation with phytosphingosine.

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TABLE 3. Heat stress and phytosphingosine causes calcineurin-dependent 4x CDRE::lacZ expression^a

A previous study showed that Slm1 is phosphorylated by the TORC2protein kinase (4). If heat stress activates phosphorylationof Slm1 and Slm2 by TORC2 and this TORC2-mediated phosphorylationis reversed by calcineurin, then in tor2^ts cells we should observeno increase in Slm1 or Slm2 phosphorylation following exposureto high temperature even in cells devoid of calcineurin activity.To test this hypothesis, we shifted wild-type or tor2^ts cellsto 37°C and then induced synthesis of either GST-Slm1 orGST-Slm2. As we observed earlier (Fig. 3), GST-Slm2 phosphorylationwas undetectable in wild-type or tor2^ts cells at 25°C, andGST-Slm1 displayed basal levels of phosphorylation that wereidentical in wild-type and tor2^ts cells (Fig. 5). We also examinedGST-Slm1 and GST-Slm2 phosphorylation in cells shifted to hightemperature in the presence of the calcineurin inhibitor FK506.As expected, phosphorylation of both proteins increased as aresult of exposure to high temperature, and we observed thesame level of phosphorylation in wild-type and tor2^ts FK506-treatedcells (Fig. 5). Thus, these findings suggest that heat stresscauses an increase in Slm1 and Slm2 phosphorylation that isTor2p-independent and counteracted by calcineurin.

Because heat stress-induced phosphorylation of Slm1 and Slm2was mimicked by the addition of phytosphingosine (Fig. 4), wetested whether the increased phosphorylation of GST-Slm1^PNIYIQand GST-Slm2^PEFYIE at high temperature was prevented by theaddition of myriocin, a potent inhibitor of the serine palmitoyltransferaseresponsible for catalyzing the first step in the biosynthesisof sphingolipids. Indeed, we found that more than 90% of theheat stress-induced phosphorylation of GST-Slm1^PNIYIQ and GST-Slm2^PEFYIEwas inhibited by myriocin (Fig. 6A), indicating that this increasein phosphorylation of Slm proteins is dependent on de novo sphingolipidbiosynthesis. In addition, these results suggest that sphingolipid-dependentprotein kinases are responsible for the increase in Slm1 andSlm2 phosphorylation observed (Fig. 3). We also investigatedthe effect of myriocin on the steady-state levels of GST-Slm1^PNIYIQand GST-Slm2^PEFYIE phosphorylation in cells grown at three differenttemperatures: 25°C, 30°C, and 37°C (Fig. 6B). First,we observed that the overall levels of both GST-Slm1^PNIYIQ andGST-Slm2^PEFYIE phosphorylation increased with temperature. Phosphorylationof GST-Slm2^PEFYIE was extremely low at 25°C and increaseddramatically with increasing temperature. GST-Slm1^PNIYIQ wasphosphorylated at all temperatures but showed increased phosphorylationwith increased temperature, especially 37°C. Second, ateach temperature where phosphorylation was detected, it wasdecreased by the addition of myriocin. We made similar observationsfor GST-Slm1 and GST-Slm2 in myriocin-treated cells lackingcalcineurin (cnb1 ${Delta}$ ) (data not shown). Thus, under all conditionstested, phosphorylation of Slm1 and Slm2 is dependent on denovo biosynthesis of sphingoid bases.

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FIG. 6. Myriocin inhibits phosphorylation of Slm1 and Slm2 during heat stress and steady-state growth conditions. GST-SLM2^PEFYIE (GBY116) and GST-SLM1^PNIYIQ (GBY118) were expressed in an slm1 ${Delta}$ slm2 ${Delta}$ strain. (A) Cells were grown at 25°C in selective synthetic medium for 4 h and protein expression was induced with 2% galactose. Thirty minutes before the shift from 25°C to 37°C, myriocin (2 µg/ml) was added to one set of cultures and solvent (methanol) to the other. Samples of the different cultures were taken at time points (t) just before the temperature shift and 90 min after the shift in temperature. GST fusion proteins were purified from cell extracts and subjected to SDS-PAGE and Western blotting with either an anti-phospho or an anti-GST antibody. (B) Cells were grown at either 25°C, 30°C, or 37°C in selective synthetic medium. Myriocin (2 µg/ml) was added 30 min before the cells were incubated with 2% galactose for 4 h. GST fusion proteins were purified from cell extracts and analyzed via Western immunoblotting with either an anti-phospho or an anti-GST antibody. Immunoreactive bands were quantified as described in Materials and Methods. A.U., arbitrary units.

Slm1 and Slm2 activity determines sensitivity to myriocin. We then investigated whether Slm1 and Slm2 play a physiologicalrole in sphingolipid signaling and/or metabolism. Sphingolipidsare essential for yeast cell growth and survival. Here, we usedmyriocin to investigate growth phenotypes related to deletionor overexpression of SLM1 and SLM2 (Fig. 7). Because Slm1 andSlm2 phosphorylation levels varied with temperature, we alsoexamined growth at two different temperatures: 30°C and37°C. First, we found that all strains tested were moresensitive to growth inhibition by myriocin at 37°C thanat 30°C, which necessitated the use of lower myriocin concentrationsat the high temperature (Fig. 7A, B, and C; compare left andright panels). Second, we found that strains lacking eitherSLM1 or SLM2 showed increased sensitivity to myriocin at bothtemperatures (Fig. 7A). A stronger effect was observed withdeletion of SLM1, which is more highly expressed than SLM2 (4).In contrast, we found that slm1 ${Delta}$ cells were more resistant toaureobasidin A (Fig. 7A), which inhibits Aur1, an enzyme responsiblefor the production of inositol phosphorylceramide, a complexsphingolipid (37). Incubation of cells with aureobasidin A canlead to the cellular accumulation of intermediates in the sphingolipidbiosynthesis pathway, including phytosphingosine and ceramide(59). We also increased Slm1 and Slm2 levels by expressing SLM1or SLM2 from a CEN-based plasmid under the control of theirown promoters. We found that increasing SLM1 and SLM2 copy numberconferred resistance to myriocin at either 30°C or 37°C(Fig. 7B). Taken together, these data implicate Slm1 and Slm2in sphingolipid metabolism and/or signaling. We then testedwhether the presence or the absence of the calcineurin-bindingsite on Slm1 and Slm2 affected resistance to myriocin (Fig.7C). At 30°C, cells expressing SLM1^PNIYIQ were more sensitiveto myriocin than cells expressing SLM1, while at 37°C, surprisingly,there was no difference in the growth rates of these two strainsover a range of myriocin concentrations (Fig. 7B and data notshown). Similarly, cells expressing SLM2^PEFYIE were more sensitiveto myriocin than cells expressing SLM2. In this case, however,the difference in growth was more dramatic at 37°C thanat 30°C. We observed equivalent effects on growth usingcells that expressed GFP-tagged versions of these proteins anddetermined that the expression level of the GFP-tagged proteinswas unaffected by the presence or absence of the calcineurin-bindingsite (data not shown). Thus, we conclude that the growth differencesdescribed above reflect calcineurin-dependent differences inSlm protein activity in vivo.

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FIG. 7. Slm1 and Slm2 modulate growth of yeast in the presence of drugs that perturb sphingolipid biosynthesis. (A) Saturated cultures of wild-type cells (BY4741) and cells lacking either slm1 (slm1 ${Delta}$ ; VHY66) or slm2 (slm2 ${Delta}$ ; VHY61) were serially diluted and spotted onto YPD, YPD plus myriocin (Myr), or YPD plus aureobasidin A (AB) and grown for 2 to 4 days at either 30°C or 37°C. (B) Wild-type cells containing either pRS313 (vector; GBY160) or pRS313 expressing Slm2 (GBY161) and Slm1 (GBY162) under the control of their own promoters were grown to saturation in selective synthetic medium. Saturated cultures were serially diluted and were spotted onto YPD with or without myriocin. Plates were incubated at either 30°C or 37°C for 2.5 days. (C) slm1 ${Delta}$ slm2 ${Delta}$ cells expressing SLM2 (GBY100), SLM2^PEFYIE (GBY101), SLM1 (GBY102), or SLM1^PNIYIQ (GBY103) under the control of their own promoters from pRS313 were grown to saturation in selective synthetic medium. Saturated cultures were serially diluted and were spotted onto YPD or YPD supplemented with 1.5 µg/ml myriocin. Cells were grown for 3 to 4 days at either 30°C or 37°C as indicated.

These data show that Slm protein activity becomes rate limitingfor yeast growth when cellular levels of sphingolipids are reducedand suggest that dephosphorylation of Slm1 and Slm2 by calcineurinis necessary for these proteins to be fully functional.

Slm proteins may act downstream of phytosphingosine. The observation that slm1 ${Delta}$ cells are both more sensitive to myriocinand more resistant to aureobasidin A than wild-type cells suggeststhat Slm proteins may be effectors of an intermediate in thesphingolipid biosynthesis pathway, such as phytosphingosine.However, our results do not rule out a role for Slm proteinsin regulating sphingolipid levels. In order to address the potentialrole of Slm proteins upstream of sphingolipids, we investigatedwhether an external source of phytosphingosine promotes cellgrowth in the absence of functional Slm proteins. Addition ofphytosphingosine (up to 20 µM) to the growth medium didnot overcome the growth defect of slm1^ts slm2 ${Delta}$ cells at the nonpermissivetemperature (38.5°C) (Fig. 8), suggesting that these cellsare defective in sphingolipid-mediated cellular processes ratherthan in sphingolipid production. In contrast, exogenously addedphytosphingosine overcame the myriocin-induced growth defectof wild-type cells at 38.5°C (Fig. 8), indicating that phytosphingosineis able to promote growth in the absence of de novo sphingolipidbiosynthesis at this high temperature. In addition, we observedthat phytosphingosine restores the myriocin-induced growth inhibitionin slm1 ${Delta}$ cells as well as in slm2 ${Delta}$ cells, indicating that eitherSlm1 or Slm2 protein can mediate the growth-promoting effectof phytosphingosine. Taken together, these results are consistentwith a role for Slm proteins acting downstream of phytosphingosine.

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FIG. 8. Slm proteins are downstream of phytosphingosine. Saturated cultures of wild-type (SEY6210), slm1 ${Delta}$ (AAY1602), slm2 ${Delta}$ (AAY1610), and slm1^ts slm2 ${Delta}$ (AAY1623.2) cells were serially diluted and spotted onto YPD, YPD plus 20 µM phytosphingosine (PHS), YPD plus 0.4 µg/ml myriocin, or YPD plus 0.4 µg/ml myriocin plus 20 µM phytosphingosine and grown for 2.5 days at the indicated temperatures. All plates contained 0.05% NP-40, which was used for obtaining even distributions of phytosphingosine in the plates.

Slm proteins are required for heat stress-induced endocytosis of the Fur4 uracil permease. Increased phytosphingosine levels disrupt yeast cell growthby inhibiting nutrient uptake, including the import of tryptophan,uracil, leucine, and histidine (14). The mechanism of this inhibitionhas been elucidated for the uracil permease, Fur4, which undergoesubiquitin-dependent endocytosis and transport to the vacuole,where it undergoes proteolysis. This degradation of Fur4 alsooccurs in response to heat stress (73) and is mediated by aspecific increase in phytosphingosine (13). We compared Fur4turnover in wild-type cells (SEY6210.1) to that in slm1^ts slm2 ${Delta}$ cells (AAY1623.2) during heat stress (Fig. 9). Since endogenousFur4 levels are too low to detect by Western blotting, we overexpressedFur4 in these cells. Cells were grown to log phase and shiftedfrom 25°C to 40°C. This temperature was used as theheat stress condition in these experiments because Fur4 turnoverwas more dramatic at 40°C than at 37°C in this strainbackground. However, we observed similar trends in Fur4 turnoverat both temperatures (data not shown). In wild-type cells, heatstress induced a time-dependent decrease in Fur4 protein levels,which is consistent with previous results (13, 73). In contrast,Fur4 levels were stable in slm1^ts slm2 ${Delta}$ cells during prolongedincubation at high temperature (Fig. 9A). This demonstratesthat Slm proteins are required for Fur4 turnover induced byheat stress. Then, we tested whether this process was modulatedby the presence or absence of the calcineurin-binding site ofSlm1 or Slm2. We compared the Fur4 turnover rate for slm1 ${Delta}$ slm2 ${Delta}$ cells expressing GST-Slm2 to that for slm1 ${Delta}$ slm2 ${Delta}$ cells expressingGST-Slm2^PEFYIE and found that Fur4 was degraded more rapidlyin cells expressing GST-Slm2^PEFYIE (Fig. 9B). A similar resultwas obtained when cells were incubated with phytosphingosine(Fig. 9C). This indicates that heat stress-induced dephosphorylationof Slm2 by calcineurin slows the rate of Fur4 turnover. Theobserved difference in turnover rates may reflect an alterationin one or more steps in the ubiquitin-dependent endocytosisand trafficking of Fur4 to the vacuole. These findings suggestthat calcineurin can regulate sphingolipid-mediated processesthrough dephosphorylation of Slm2. However, we observed no differencein Fur4 turnover rates in cells expressing GST-Slm1 versus GST-Slm1^PNIYIQ(data not shown).

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FIG. 9. Slm function is required for heat shock-induced Fur4 turnover. (A) Wild-type cells (SEY6210.1) and slm1^ts slm2 ${Delta}$ cells (AAY1623.2) carrying pVTu-FUR4 (GBY179 and GBY180, respectively) were shifted from 25°C to 40°C and samples were taken at time points (t) just prior to (0 min) and 15, 30, and 60 min after heat shock. Cell lysates were analyzed by SDS-PAGE and immunoblotting with anti-Fur4 and anti-PGK antibodies. Pgk1 was used as a loading control, which also shows the absence of nonspecific protein degradation by heat shock. The numbers to the left of the gels indicate the molecular masses of the protein standards. Immunoreactive bands were quantified as described in Materials and Methods. The ratio of the anti-Fur4 signal to the anti-Pgk1p signal is shown as a function of time. The value at 0 min was used as the reference value and set at 100%. (B) slm1 ${Delta}$ slm2 ${Delta}$ cells expressing either GST-SLM2 or GST-SLM2^PEFYIE and overexpressing FUR4 (GBY115 and GBY116, respectively) were shifted from 25°C to 40°C and sampled at the indicated time points. Cell lysates were analyzed by immunoblotting and quantified as described for panel A. (C) GBY115 and GBY116 were grown at 30°C, incubated with 20 µM phytosphingosine, and sampled at the indicated time points. Lysates were analyzed and signals quantified as described for panel A.

Next, we examined in more detail the accumulation of Fur4 inslm^ts cells. We included cycloheximide during the incubationat high temperature to follow only the fate of presynthesizedFur4 (73). We also assayed Fur4 levels by monitoring [¹⁴C]-uraciluptake (Fig. 10A), which allows sensitive quantification ofcell surface Fur4, as any Fur4 in intracellular compartmentswill not contribute to uracil transport. As previously described,after a shift to high temperature, uracil uptake rapidly decreasedin wild-type cells (73). In contrast, uracil transport activityremained high in slm^ts cells. These observations establish thatinternalization of Fur4 is blocked in slm^ts cells at restrictivetemperature. It has been shown that, as for many membrane proteins,ubiquitination of Fur4 precedes and is required for its internalization(31). Using the anti-Fur4 antibody, we showed that in plasmamembrane fractions of slm^ts cells exposed to high temperature,Fur4 accumulates in high-molecular-weight forms (Fig. 10B).These slow-migrating forms of Fur4 were also seen in plasmamembrane fractions of act1-3 cells at restrictive temperature,which are defective for endocytosis and have been shown to accumulateubiquitinated forms of Fur4 (reference 31 and Fig. 10B). Incontrast, high-molecular-weight forms of Fur4 were not observedin mutants defective for the Rsp5 ubiquitin protein ligase,which is responsible for cell surface ubiquitylation of Fur4and many other plasma membrane proteins (reference 31 and Fig.10B). Membrane fractions of slm^ts and act1-3 cells incubatedat restrictive temperature also accumulated high-molecular-weightspecies that reacted with an anti-ubiquitin antibody (data notshown). Therefore, we conclude that in slm^ts cells, Fur4 accumulatesat the plasma membrane in a ubiquitinated form and that internalizationis inhibited at a postubiquitination step.

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FIG. 10. Fur4 is stabilized at the plasma membrane in the ubiquitinated form in cells lacking Slm protein activity. Wild-type cells (SEY6210.1) and slm1^ts slm2 ${Delta}$ cells (AAY1623.2) carrying pVTu-FUR4 (GBY179 and GBY180, respectively) were shifted to 40°C for 10 min before the addition of cycloheximide (100 µg/ml). (A) Uracil uptake was measured at the times indicated. Results are percentages of initial activities. (B) Plasma membrane fractions were prepared from cycloheximide-treated cells before and 60 min after a shift from 25°C to 40°C and analyzed for uracil permease (anti-Fur4) by Western immunoblotting. Strains are as follows: left panel, wild type (wt) (SEY6210.1) and slm^ts (AAY1623.2); middle panel, wild type (NY13) and act1-3 (NY279); right panel, wild type (FY56) and rsp5^ts (FW1808).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The major finding of this study is that Slm1 and Slm2 are novelcalcineurin substrates that promote yeast cell growth undersphingolipid-limiting conditions and endocytosis of a nutrientpermease in response to heat stress. Interfering with calcineurin-dependentdephosphorylation of Slm proteins alters their activity in vivo.Thus, these studies identify a mechanism by which calcineurinmay modulate sphingolipid-dependent events and establish thepotential for cross talk between these two signaling pathways.

Slm1 and Slm2 are novel calcineurin substrates. In this study, we identify Slm1 and Slm2 as targets of the phosphatasecalcineurin and show that, like other calcineurin substrates(1, 3, 18, 36, 66), Slm1 and Slm2 each contain a PXIXIT-relateddocking site that mediates its interaction with the A subunitof calcineurin. This interaction is essential for dephosphorylationof Slm1 and Slm2 by calcineurin, and by creating SLM1 and SLM2alleles lacking their respective PXIXIT motifs, we were ableto assess the contribution of calcineurin signaling to Slm1and Slm2 function in vivo.

Slm1 and Slm2 bind to calcineurin with different affinities.In vivo yeast two-hybrid assays suggest that full-length Slm2associates more tightly with calcineurin than Slm1 does, andin vitro assays confirm this difference (J. Roy, H. Li, P. G.Hogan, and M. S. Cyert, unpublished results). Furthermore, theaffinities of Slm1 and Slm2 for calcineurin correlate with theextents to which they are dephosphorylated by this phosphatase.Slm2 is completely dephosphorylated by calcineurin in vivo andin vitro, while Slm1 is only partially dephosphorylated by calcineurin.

The physiological consequences of calcineurin-mediated Slm dephosphorylationhave yet to be fully elucidated. SLM1 and SLM2 are redundantfor an essential function, which does not require calcineurin,as SLM1^PNIYIQ and SLM2^PEFYIE each support viability. In cellsexpressing a single SLM allele, however, abrogating Slm2 regulationby calcineurin modifies its function: the ability of Slm2^PEFYIEto promote growth in the presence of myriocin is compromised,and expression of this protein causes faster turnover of theFur4 permease during heat stress. Disruption of Slm1 regulationby calcineurin also diminishes its ability to support myriocinresistance at 30°C but has no effect on Fur4 turnover. Takentogether, these observations indicate that calcineurin can modifySlm function. However, in wild-type cells, which express bothSlm1 and Slm2 and in which Slm1 is the predominant protein (4),the physiological significance of this regulation is somewhatunclear. Calcineurin, which is activated under conditions ofenvironmental stress, may modify a specific aspect of Slm functionor a restricted population of Slm proteins under these conditions.Further investigation is required to establish the biochemicalmechanism by which Slm proteins act and, similarly, to fullyappreciate the consequences of their dephosphorylation by calcineurin.

Slm proteins may act downstream of sphingoid bases. Sphingolipids are produced via a pathway that is conserved fromyeast to mammals (20, 60). They consist of a long-chain base,which is usually a linear alkane of 18 or 20 carbons havinghydroxyls on C-1 and C-3 and an amino group on C-2. Yeast makestwo types of long-chain bases, dihydrosphingosine and phytosphingosine.These sphingoid bases rapidly and transiently accumulate duringheat stress but are not incorporated into ceramides or complexsphingolipids (60). Rather, they act as signals to promote cellularstress responses. Importantly, addition of exogenous sphingoidbases to yeast at low temperature induces several aspects ofthe heat stress response, including trehalose accumulation,the expression of stress element (STRE)-controlled stress responsegenes, cell cycle arrest, and the stimulation of ubiquitin-dependentprotein turnover (13, 21, 44, 58, 76). Sphingoid bases exerttheir effects at least in part by activating protein phosphorylation(12, 41, 29).

Our data suggest a possible role for Slm proteins as mediatorsof sphingolipid-dependent signaling. First, phosphorylationof Slm1 and Slm2 is modulated by sphingoid bases in vivo. Second,Slm proteins are required for heat stress-induced turnover ofthe Fur4 permease, which is induced by sphingoid bases (13).Third, Slm1 and Slm2 modulate cell growth in the presence ofdrugs that perturb sphingolipid biosynthesis. Fourth, in contrastto lcb1-100 cells, which are defective in the first step ofsphingolipid biosynthesis (76), the lethality of cells lackingSlm protein activity is not overcome by providing an externalsource of phytosphingosine, suggesting that Slm proteins actdownstream of this mediator.

Phosphorylation of Slm proteins is modulated by sphingolipids. The biochemical function of Slm1 and Slm2 is yet to be elucidated;however, it is clear that their activity and phosphorylationare highly regulated in vivo. Our studies examine modulationof Slm protein phosphorylation by sphingolipids and the proteinphosphatase calcineurin during both heat stress and growth atconstant temperature. During heat stress, a major consequenceof increased levels of phytosphingosine and dihydrosphingosineis activation of protein kinases. Pkh1 and Pkh2, the yeast homologsof mammalian PDK1 (12), are activated by phytosphingosine andin turn phosphorylate and activate downstream kinases, includingYpk1, Ypk2, Pkc1, and Sch9 (12, 41, 61). Some of these kinases(Ypk1, Ypk2, Sch9) may also be stimulated directly by phytosphingosine(52). Heat stress and exogenous addition of sphingoid basesalso stimulate calcineurin activity (reference 78 and Table3). The mechanism for this activation must still be uncoveredbut is likely to involve stimulation of Ca²⁺-influx systems,as exposure of yeast cells to sphingosine L-phosphate, a sphingolipidproduced in mammalian cells, stimulates Ca²⁺ accumulation (8).

When cells are shifted to high temperature, the net level ofSlm1 and Slm2 phosphorylation changes little over the next 75min. However, during this time, there is enhanced sphingolipid-dependentphosphorylation of Slm proteins that is counteracted by calcineurin-mediateddephosphorylation. Thus, during heat stress, the rate at whichSlm1 and Slm2 cycle between their phosphorylated and dephosphorylatedstates must increase. Currently, it is unclear what consequencethese changes in phosphorylation state have on Slm protein function.Perhaps, as for small GTP-binding proteins, the switch betweentwo different states is an integral aspect of Slm protein activity.

Additional studies are required to establish which kinase orkinases are responsible for the heat stress-induced phosphorylationof Slm proteins. Kinases that are activated by phytosphingosinedirectly (Pkh1, Pkh2, Ypk1, Ypk2, and Sch9) or indirectly (Pkc1)are attractive candidates. A recent study showed that myriocintreatment abrogates Mss4-dependent PIP kinase activity (47),which might in turn reduce recruitment of Slm proteins to theplasma membrane, which depends on PIP₂ binding to the PH domainin each protein (4). Thus, sphingolipids may also affect Slmprotein phosphorylation indirectly by modulating their localizationand access to kinases that reside at the cell periphery, suchas Tor2p. Consistent with this possibility, we observed an increasein cytosolic localization of GFP-Slm1 and GFP-Slm2 in myriocin-treatedcells (data not shown).

A previous study showed that TORC2 phosphorylates Slm1 in vitro(4). Furthermore, pulse-chase analysis of Slm1 revealed itsrapid dephosphorylation after exposure to high temperature,followed by TOR2-dependent rephosphorylation. The timing ofthese events parallels that of the transient delocalizationof the actin cytoskeleton in response to heat stress. In contrast,by analyzing steady-state phosphorylation of the entire cellularpool of Slm1 and Slm2, we observe a heat stress-induced increasein phosphorylation that is independent of Tor2p and occurs overa prolonged time period ( $≥$ 75 min) when calcineurin is inactivated.These kinetics are more similar to that of downstream eventssuch as endocytosis of Fur4, which continues $≥$ 120 min followinga shift to high temperature. It is likely, then, that multiplephosphorylation events occur, with both Tor2p and sphingolipid-regulatedkinases contributing to total phosphorylation of Slm proteinsduring heat stress and potentially playing quite different rolesin Slm regulation. Sphingolipid-dependent phosphorylation ofSlm1 and Slm2 that is counteracted by calcineurin is also observedin cells grown under constant conditions, with the extent ofSlm phosphorylation increasing with temperature. Thus, similarprocesses may underlie Slm protein phosphorylation during bothnormal and stress conditions.

Slm proteins are required for heat stress-induced Fur4 endocytosis. Sphingolipids inhibit nutrient import during heat stress bypromoting degradation of nutrient permeases, including the uracilpermease, Fur4, and the general amino acid permease, Gap1 (13,14). This degradation depends on the de novo biosynthesis ofsphingolipids and is mimicked by the addition of exogenous phytosphingosine(13). Slm proteins are required for heat stress-induced Fur4turnover, which occurs through ubiquitination, internalization,and trafficking of the permease to the vacuole (9, 25, 26, 30,31). Ubiquitinated Fur4 accumulates at the surface of slm1^tscells, indicating that Slm proteins are required for internalizationof Fur4. The actin cytoskeleton is required for the internalizationstep of endocytosis; many mutants with defects in actin organizationor actin-binding proteins are unable to carry out endocytosisand accumulate ubiquitylated forms of Fur4 at the cell surface(31, 46, 57). Furthermore, mutants that lack components of theendocytosis machinery, such as the amphiphysin homologs, Rvs161and Rvs167, are defective for actin polarization (54). slm1^tscells show defects in both actin cytoskeleton polarization (4)and endocytosis and may therefore participate directly in eitheror both of these processes.

A role for sphingolipid signaling in endocytosis has been clearlydemonstrated by studies of lcb1-100<