t-SNARE Phosphorylation Regulates Endocytosis in Yeast

doi:10.1091/mbc.01-11-0541

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Originally published as MBC in Press, 10.1091/mbc.01-11-0541 on February 28, 2002

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Vol. 13, Issue 5, 1594-1607, May 2002

t-SNARE Phosphorylation Regulates Endocytosis in Yeast

Sangiliyandi Gurunathan, Michael Marash, Adina Weinberger, and Jeffrey E. Gerst^*

Department of Molecular Genetics, Weizmann Institute of Science, Rehovot 76100, Israel

Submitted November 7, 2001; Revised January 28, 2002; Accepted February 1, 2002
Monitoring Editor: Randy Schekman

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Earlier we demonstrated that activation of a ceramide-activated protein phosphatase (CAPP) conferred normal growth and secretionto yeast lacking their complement of exocytic v-SNAREs (Snc1,2)or bearing a temperature-sensitive mutation in an exocytic t-SNARE(Sso2). CAPP activation led to Sso dephosphorylation and enhancedthe assembly of t-SNAREs into functional complexes. Thus, exocytosisin yeast is modulated by t-SNARE phosphorylation. Here, we showthat endocytic defects in cells lacking the v- and t-SNAREs involvedin endocytosis are also rescued by CAPP activation. Yeast lackingthe Tlg1 or Tlg2 t-SNAREs, the Snc v-SNAREs, or both, undergoendocytosis after phosphatase activation. CAPP activation correlatedwith restored uptake of FM4-64 to the vacuole, the uptake anddegradation of the Ste2 receptor after mating factor treatment,and the dephosphorylation and assembly of Tlg1,2 into SNARE complexes.Activation of the phosphatase by treatment with C₂-ceramide, VBM/ELOgene inactivation, or by the overexpression of SIT4 was sufficientto confer rescue. Finally, we found that mutation of single PKAsites in Tlg1 (Ser31 to Ala31) or Tlg2 (Ser90 to Ala90) was sufficientto restore endocytosis, but not exocytosis, to snc cells. Theseresults suggest that endocytosis is also modulated by t-SNAREphosphorylation invivo.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Intracellular protein and lipid trafficking involves the selective transfer of cargo molecules from one compartment to thenext. This is accomplished by the fusion of membranes derivedfrom the donor compartment with those belonging to a specifictarget. A number of proteins are involved in the tethering, docking,and fusion steps that confer bilayer fusion and subsequent proteintransport. Among those, SNAREs comprise three evolutionarily conservedfamilies (e.g., the syntaxin, synaptobrevin/VAMP, and SNAP-25families) of membrane-associated proteins that are required forthe docking and fusion steps (Ferro-Novick and Jahn, 1994; Rothmanand Warren, 1994). On encroachment to the target compartment,SNAREs from the donor or vesicular membranes (v-SNAREs) form complexesin trans with cognate SNARE partners from the opposing targetmembrane (t-SNAREs). The SNARE complex usually involves threeor four SNARE molecules, each contributing one or two $alpha$ -helicalcores to the formation of a four-helix coiled-coil bundle (Suttonet al., 1998; Katz et al., 1998). Formation of this complex isnecessary and sufficient for membrane fusion in vitro but necessitatesinteractions between specific and precisely arrayed SNARE partners(Weber et al., 1998; McNew et al., 2000).

Because SNAREs play a pivotal role in the fusion process, it is likely that they receive input from the cellular environmentto either enhance or impede membrane trafficking events. In particular,kinases involved in growth control are likely to modulate SNAREfunctions, presumably by the posttranslational modification ofresidues that participate in SNARE partnering or the binding ofSNARE regulatory proteins (reviewed in Gerst, 1999; Turner etal., 1999; Klenchin and Martin, 2000). Numerous studies have outlinedthe possible involvement of kinases in the regulation of SNAREprotein interactions (Hirling and Scheller, 1996; Shimazaki etal., 1996; Foster et al., 1998; Shuang et al., 1998; Risingerand Bennett, 1999; Chung et al., 2000) as well as the availabilityof SNAREs to participate in membrane trafficking events (Cabaniolset al., 1999; Foletti et al., 2000; Kataoka et al., 2000). Therefore,a role for signal-induced protein kinases in regulating SNAREcomplex assembly is likely and offers a potential mechanism forcoordinating the dynamics of cell growth with cell cyclecontrol.

In yeast, the Snc v-SNAREs (Gerst et al., 1992; Protopopov et al., 1993) assemble into fusion complexes with the Sso and Sec9t-SNAREs to form the exocytic SNARE complex (Brennwald et al.,1994; Couve and Gerst, 1994; Rossi et al., 1997). Deletion ofthe SNC genes results in the intracellular accumulation of secretoryvesicles, in an inhibition in protein secretion, and in variousconditional lethal phenotypes (Protopopov et al., 1993; Davidet al., 1998). Mutations in either of two genes that encode homologousER-localized proteins (Vbm1,2/Elo2,3), which are involved in long-chainfatty acid (LCFA) elongation, result in the intracellular accumulationof phytosphingosine and rescue snc cells (David et al., 1998).This occurs via activation of a sphingoid base/ceramide-activatedphosphatase (CAPP), Sit4, and the subsequent dephosphorylationof discrete PKA sites in the Sso t-SNAREs (Marash and Gerst, 2001).Thus, two signal transduction pathways in yeast converge uponthe exocytic t-SNAREs and have opposing effects on their abilityto form SNARE complexes. The PKA pathway, which is involved ingrowth control, phosphorylates Sso proteins and inhibits theirassembly into SNARE complexes in vitro and in vivo. In contrast,a CAPP signaling pathway, which mediates cellular stress responses,activates Sit4 and dephosphorylates the Sso t-SNAREs. Dephosphorylationof the t-SNAREs enhances SNARE complex assembly and led to restoredsecretion in cells bearing mutations in the Snc v-SNAREs or Ssot-SNAREs (Marash and Gerst, 2001).

The Snc exocytic v-SNAREs also mediate endocytosis (Gurunathan et al., 2000). In snc null cells or cells possessing a temperature-sensitiveallele of SNC1 (snc1^ala43) that were shifted to restrictive temperatures, uptake of thesoluble dye FM4-64 and the Ste2 mating factor receptor to thevacuole is abolished. Thus, Snc v-SNAREs confer both anterogradeand retrograde transport events between the Golgi and the plasmamembrane. Appropriately, their endocytic functions are likelyto be dependent on two different t-SNAREs, Tlg1 and Tlg2, whichare trans-Golgi and endosomal t-SNAREs involved in endosomal proteinsorting (Abeliovich et al., 1998; Holthuis et al., 1998a; Seronet al., 1998; Coe et al., 1999; Abeliovich et al., 1999). Thisis because Snc proteins coimmunoprecipitate with the Tlg t-SNAREs(Abeliovich et al., 1998; Holthuis et al., 1998a); Snc1^ala43 is nonfunctional in their absence (Gurunathan et al., 2000);and snc tlg1 and snc tlg2 strains show synthetically enhancedphenotypes (Gurunathan et al., 2000). Moreover, Tlg1 and 2 havebeen recently shown to bind Snc v-SNAREs and to mediate an invitro fusion event similar to endocytosis (Paumet et al., 2001).

Here we show that CAPP activation also confers normal endocytic functioning to cells lacking the Snc v-SNAREs. Rescue occursby either the exogenous treatment of cells with active ceramideanalogs, by VBM gene inactivation, or by overexpression of SIT4itself. Interestingly, endocytic defects in cells lacking eitherTlg1 or Tlg2 alone or in combination with deletions in the SNCgenes are also rescued by CAPP activation. In all cases, rescuecorrelated with the dephosphorylation of Tlg1 and Tlg2 and theirassembly into complexes both in vivo and in vitro. Finally, wedemonstrate that the mutation of single PKA sites in the putativeNH₂-terminal auto-inhibitory domains of Tlg1 and Tlg2 resultsin constitutively activated SNAREs that confer endocytosis inthe absence of CAPP activation. Thus, both the PKA and CAPP signalingpathways modulate endocytosis by regulating phosphorylation ofthe Tlg t-SNAREs and their ability to assemble into SNAREcomplexes.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Media, DNA, and Genetic Manipulations

Yeast were grown in standard growth media containing either 2% glucose or 3.5% galactose. Synthetic complete (SC) and dropoutmedia similar to that described (Rose et al., 1990) were prepared.Standard methods were used for the introduction of DNA into yeastand the preparation of genomic DNA (Rose et al., 1990).

Growth Tests

Yeast were grown on synthetic and rich growth media (Rose et al., 1990). In experiments involving ceramide, N-acetyl-D-erythro-sphingosine(C₂-ceramide; Sigma, St. Louis, MO) was dissolved in ethanol (at15 mM or 1 mg/ml) and added to the media to a final concentrationof 10 µM. For growth tests on plates, yeast were counted usinga hemocytometer, diluted serially, and plated by drops onto solidmedium preincubated at different temperatures. For growth of cellsin liquid culture, cells were cultured overnight in medium containingC₂-ceramide.

For growth tests involving snc and snc tlg mutants, which carry a galactose-inducible form of SNC1, cells were grown to logphase on galactose-containing synthetic medium. Next, cells wereshifted to glucose-containing medium (36 h) to induce the sncphenotype. Cells were then seeded at an optical density (OD₆₀₀)of 0.05 into fresh glucose-containing medium at 26°C with or withoutthe addition of 10 µM C₂-ceramide. Cells were monitored for growth(OD measured at 600 nm) every 3 h up to 36 h. Saturation of theculture (with or without ceramide) was reached usually by 27 h.OD₆₀₀ values were plotted on graphs versus time to show the kineticsof saturation as well as on logarithmic graphs to calculate celldivision times for the differentstrains.

For growth tests involving snc1^ala43 and snc1^{ala43 tlg} cells, cells were grown to log phase on glucose-containing medium at 26°C. Cellswere then seeded at an OD₆₀₀ of 0.05 into prewarmed glucose-containingmedium either containing or lacking C₂-ceramide (10 µM) and grownat 37°C. Cells were monitored for growth as describedabove.

Yeast Strains

Yeast strains used are listed in Table 1. To create snc tlg vbm1 yeast, the snc vbm1 strains DD1 and MM1 were cured of theirGAL-SNC1-containing plasmids and transformed with linearized DNAfragments isolated from the enzymatic digestion of pTLG1L andpTLG2T (Gurunathan et al., 2000). Transformants were selectedand the disruptions verified by PCR analysis. To create snc1^ala43 tlg yeast, snc tlg cells (JG9-TLG1 or JG9-TLG2) were transformedwith either plasmid pLADH-SNC1^ala43 or pTADH-SNC1^ala43. Transformants were cured of their GAL-SNC1-containing plasmidson synthetic medium at 26°C. For cells expressing STE2-GFP constructsthat bear the kan^r resistance marker, strains were transformed with YCpKSTE2-GFPand selected for on synthetic medium containing 100 µg/ml geneticin.

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Table 1. Strains used in this study

Plasmids

Previously described SNC expression plasmids included the following: pADH-SNC1 (Gerst et al., 1992); pADH-HASNC1 and pTGAL-SNC1(Protopopov et al., 1993); and pAHGAL-SNC2 (David et al., 1998).Plasmids pRS314STE2-GFP and pRS314ste2 $Delta$ tail-GFP, which expressthe STE2-GFP or STE2-tailGFP gene fusions (Stefan and Blumer,1999), respectively, were provided by K. Blumer (Washington UniversitySchool of Medicine). snc1^ala43 expression constructs included: pADH-SNC1^ala43; pTADH-SNC1^ala43; and pLADH-SNC1^ala43 (Gurunathan et al., 2000). TLG1,2 disruption constructs, pTLG1Land pTLG2T, respectively, were described previously, as was aCEN plasmid that expresses STE2HA, pLADH-STE2HA (Gurunathan etal., 2000). Plasmids for the expression of SIT4 (YEpSIT4) in yeastand TPK1 (pGEX-TPK1) in bacteria were described previously (Marashand Gerst, 2001). Plasmids created for this study are listed inTable 2.

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Table 2. Plasmids created for this study

Microscopy

Cells were labeled with FM4-64 and monitored for fluorescence, as described (Gurunathan et al., 2000). GFP fluorescence wasvisualized via the FITC channel in strains expressing the appropriateGFP fusion proteins. Thin sectioning and electron microscopy wasperformed essentially as described by Zelicof et al. (1996). Quantificationof the vesicles per unit area was calculated by counting the numberof vesicles in photos of thin-sectioned cells. Next, the totalarea counted was determined by weighing cutouts of the cells anddividing them by the weight of a cutout equivalent to 1 µm². Dividing the former by the latter yields the number of vesiclesper µm². At least 30 cells per strain were used in themeasurements.

Metabolic Labeling

Pulse-chase studies for Ste2 uptake, using [³⁵S]methionine (Amersham, Amersham, United Kingdom), were performed essentiallyas described previously (Hicke and Riezman, 1996). snc cells grownon galactose-containing medium at 26°C were shifted to glucose-containingmedium for 30 h before pulse-labeling (30 min) with [³⁵S]methionine (0.1 mCi/OD₆₀₀ unit). After a 30-min chase in mediumcontaining 5 mM methionine and cysteine, cells were treated with $alpha$ -factor (1 µM) for up to 60 min. Cell extracts were prepared,and Ste2HA was immunoprecipitated using anti-HA antibodies. PrecipitatedSte2HA was solubilized in SDS-containing sample buffer, heatedfor 15min at 37°C, and resolved on 10% SDS-PAGE gels. For experimentsinvolving snc1^ala43 cells at 37°C, strains were shifted to 37°C 1 h beforelabeling.

SNARE Complex Measurement from Cell Lysates

SNARE complexes present in cell lysates were monitored by the immunoprecipitation (IP) of SNAREs from cell extracts, as describedin Couve and Gerst (1994). However, the following additions tothe lysis and IP buffers were made: 0.5% NP-40 (instead of TritonX-100); MG132 (100 µM), ATP $gamma$ S (20 µM), EDTA (2 mM), and n-ethylmaleimide(1 mM), to inhibit SNARE complex dissociation and degradation.Anti-Tlg1 and anti-Tlg2 antibodies (gifts of H. Pelham and H.Abeliovich) were used for IP (1 µl per reaction) and detection(1:2000). The amount of Tlg1 present in heteromeric complexeswith Tlg2 was determined using the anti-Tlg2 antiserum for IPand detection with the anti-Tlg1 antiserum. The presence of Tlg1or Tlg2 in homomeric complexes were determined by expressing myc-taggedTlg1 or Tlg2 in snc tlg2 and snc tlg1 cells, respectively. IPwas performed using anti-myc antibodies (Santa Cruz Biotechnology,Santa Cruz, CA), and subsequent detection of both tagged and untaggedproteins was performed using anti-Tlg1 or anti-Tlg2 antibodies.Samples of TCLs, and immunoprecipitates were resolved by electrophoresisand detected by Western blotting. Detection was performed usingchemiluminescence(ECL).

Measurement of Tlg Phosphorylation and SNARE Assembly In Vitro

Recombinant GST fusions of Tlg1 and 2, Tpk1, and Sit4 were expressed separately in BL21 Escherichia coli and purified overglutathione-Sepharose beads, using standard procedures. Affinity-purifiedGST-Tlg1^1-206 and GST-Tlg2^1-317 were phosphorylated in vitro by Tpk1, using the procedure describedpreviously for GST-Sso1^1-265 (Marash and Gerst, 2001). Labeled proteins were detected in SDS-PAGEgels using autoradiography or by protein-dye staining using Coomassieblue (Bio-Rad Laboratories, Richmond, CA). To measure dephosphorylation,recombinant GST-Sit4 (2 µg) or GST-Sit4 (2 µg) with C₂-ceramide(0.05 mM) was added. To measure the association of Tlg1 and Tlg2,affinity-purified in vitro phosphorylated or nonphosphorylatedGST-Tlg1^1-206 and GST-Tlg2^1-317 proteins were mixed together at a ratio of 1:1 (5 µg each) inbuffer containing 0.5% Triton X-100 in PBS and allowed to incubateovernight at 4°C. After which, the proteins were IP'd with anti-Tlg1(1 µl per IP reaction), resuspended in sample buffer, and resolvedby SDS-PAGE. Detection and quantification of the proteins usingeither anti-Tlg1 or -Tlg2 antibodies (1:2000 dilution) was performedusing ECL. ECL signals were measured over a linear range of activity,as determined using known quantities of recombinant GST-Tlg proteinsas standards in Westernblots.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

vbm Mutation or the Exogenous Addition of C₂-ceramide Rescue Growth Defects in snc, snc tlg, and Temperature-shifted snc1^ala43 and snc1^ala43 tlg Cells

Previous work demonstrated that defects in exocytosis in snc null cells or cells bearing a temperature-sensitive mutationin the Sso2 t-SNARE can be rescued by the exogenous addition ofactive sphingoid bases and ceramide analogs to the growth medium.These molecules activate CAPP and mimic the effects seen uponvbm gene mutation in snc yeast, leading to dephosphorylation ofthe Sso t-SNAREs. Because the Snc v-SNAREs are also involved inendocytosis, we determined whether the exogenous addition of C₂-ceramide,an active form of ceramide, or vbm gene mutation can restore normalendocytic trafficking in snc cells. We also wanted to test itseffects on snc tlg1 and snc tlg2 yeast, which lack one of theTLG genes and are more growth deficient than snc cells. Becausethe snc and tlg mutations each block endocytic functioning, itis likely that the synthetic phenotypes observed in the triplemutants result from an additional role for Tlg1 and 2 in anterogradetransport (Gurunathan et al., 2000).

First, it was important to determine the effects of ceramide addition or vbm mutation on the growth of snc tlg cells to showwhether cells lacking both v- and t-SNAREs are rescued (Table3). Cells were grown at 26°C in liquid culture in glucose-containingmedium in order to shut off SNC1 expression from under a galactose-induciblepromoter. In the absence of SNC1 expression, snc and snc tlg cellsgrew slowly and had doubling times of ~4 h, whereas snc cellsconstitutively expressing SNC1 double every 2 h. In contrast,snc and snc tlg cells treated with ceramide had shorter doublingtimes of 2.4 h and ~3 h, respectively. Introduction of a vbm1/elo3mutation in snc tlg yeast had a similar effect and lowered thedoubling time to ~2 h. Both snc tlg vbm1 cells and ceramide-treatedsnc tlg cells reached the same level of saturation as snc cellsconstitutively expressing SNC1 (our unpublished results). Finally,we found that snc tlg cells treated with ceramide grew much betterat other temperatures (i.e., 15°C, 30°C, 35°C, and 37°C), includingsnc tlg1 cells, which normally do not grow at 15°C and at temperatures> 26°C (Gurunathan et al., 2000; our unpublished results). Thus,both ceramide treatment and VBM gene disruption, which activateCAPP, restore growth in snc tlg cells, as shown previously forsnc cells. We note that the growth of cells bearing the tlg1 mutationwas slightly slower than that of snc tlg2 cells, even in the presenceof ceramide or after the disruption of VBM1. This correspondswith earlier results that indicate TLG1 disruption is more severethan that of TLG2 (Gurunathan et al., 2000).

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Table 3. Cell division times

We also tested whether the growth of tlg1 and tlg2 deletion mutants at 26°C is improved upon ceramide treatment or the overexpressionof SIT4. We found that tlg cells have a doubling time of ~2.2h, whereas after ceramide treatment (Table 3) or the overexpressionof SIT4 (our unpublished results) this value remained basicallythe same (2.1 h for both tlg1 and tlg2 yeast). Because the growthdefects in tlg yeast are mild, it is likely that CAPP activationhas only littleeffect.

The snc1^ala43 allele encodes a thermosensitive v-SNARE (Gurunathan et al., 2000) that is defective specifically in its retrievaland recycling from the plasma membrane (Grote et al., 2000; Gurunathanet al., 2000; Lewis et al., 2000). When expressed from a single-copyplasmid, snc1^ala43 confers the growth of snc cells up to 35°C, although the growthrate is slower than that conferred by native SNC1 (Gurunathanet al., 2000). Interestingly, the expression of snc1^ala43 in snc tlg cells does not rescue their growth defects, suggestingthat the TLG gene products are essential for Snc1^ala43 function and/or recycling (Gurunathan et al., 2000). We nextexamined the effects of ceramide addition on snc1^ala43 and snc1^ala43 tlg cells that were shifted to the restrictive temperature (37°C;Table 3). In the absence of ceramide, we found that snc1^ala43 and snc1^ala43 tlg cells were unable to grow altogether, as shown previously(Gurunathan et al., 2000). However, after ceramide treatment allstrains grew robustly at 37°C and had doubling times of ~3 h.Treated snc1^ala43 tlg yeast grew slightly slower than their snc1^ala43 counterparts (Table 3), but reached a similar final density(our unpublished results). Thus, ceramide treatment appears torestore the functionality of Snc1^ala43.

Ceramide Treatment Inhibits Vesicle Accumulation in snc tlg Cells

Secretory vesicles (SVs) are hardly seen in thin-sectioned wild-type yeast but are common in snc cells growing at permissivetemperatures (Protopopov et al., 1993; David et al., 1998). Wenext examined the accumulation of 100-120 nm SVs in ceramide-treatedand untreated snc and snc tlg cells by electron microscopy. Wecounted the number of SVs present in thin-sectioned snc tlg1 andsnc tlg2 cells and found they had 24 ± 1 and 19.0 ± 0.5 vesiclesper µm², respectively, which was similar to control snc cells (17.0 +0.7 vesicles per µm²). However, upon treatment with ceramide, the number of vesiclesper µm² declined by >60%; snc tlg1 and snc tlg2 cells had 9.0 ± 0.7 and7.0 ± 0.6 vesicles per µm², respectively. Control snc cells were found to have 5.0 ± 0.9vesicles per µm² after treatment, as shown previously (Marash and Gerst, 2001).Thus, although snc tlg cells accumulate more SVs than snc cells,their numbers are also greatly reduced upon ceramidetreatment.

Delivery of the Soluble Dye FM4-64 to the Vacuole Is Restored in snc, snc tlg, and Temperature-shifted snc1^ala43 and snc1^ala43 tlg Cells upon Ceramide Treatment or vbm Mutation

Because ceramide treatment has pronounced effects on exocytosis (i.e., cell growth and SV accumulation) in both snc and snctlg yeast, we determined whether endocytosis is restored in thesecells by the exogenous addition of C₂-ceramide. Previously, wehave shown that these strains are defective in the uptake of thevacuolar staining dye, FM4-64 (Gurunathan et al., 2000). Labelingof the cytoplasm and small vacuolar bodies was shown to occurin glucose-shifted snc cells and temperature-shifted snc1^ala43 cells as a function of time. snc tlg cells also are labeled ina similar manner, even when expressing SNC1, due to the loss inTlg functioning (Gurunathan et al., 2000).

snc and snc tlg strains were shifted to glucose-containing medium for 24 h to induce the snc phenotype. Cells were incubatedwith FM4-64 for short periods and examined in vivo using fluorescenceand visual (Nomarski) microscopy (Figure 1A). As expected, untreatedsnc cells had a hazy staining of the cytoplasm and small, fragmented,vacuolar bodies. Likewise, snc tlg1 and snc tlg2 cells had anidentical staining pattern, unlike control snc cells expressingSNC1. Ceramide treatment restored FM4-64 staining of the vacuolenot only in snc cells, but also in snc tlg cells. Moreover, largeround vacuoles were apparent in the treated cells, as observedusing Nomarski optics. These results suggest that ceramide treatmentrestores dye trafficking and vacuole biogenesis to snc cells,even in the presence of tlg mutations.

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Figure 1. Delivery of FM4-64 to the vacuole is restored in snc, snc tlg, and temperature-shifted snc1^ala43cells by CAPP activation. (A) Delivery of FM4-64 to the vacuole is restored in snc tlg cells. SNC1, snc (JG8), snc tlg1 (JG9-TLG1), and snc tlg2 (JG9-TLG2) cells were grown to log phase on galactose-containing medium, before being shifted to glucose-containing medium at 26°C for 36 h, with (+C₂) or without ( $-$ C₂) C₂-ceramide. Cells were incubated with FM4-64 (1 µg/ml) and processed for fluorescence and light (Nomarski) microscopy. (B) Delivery of FM4-64 to the vacuole is restored in snc vbm1 (MM1), snc tlg1 vbm1 (JG9-TLG1, VBM1), and snc tlg2 vbm1 (JG9-TLG2, VBM1) cells. Cells were grown on glucose-containing medium for 24 h at 26°C, incubated with FM4-64, and processed for microscopy. (C) Delivery of FM4-64 to the vacuole is restored in ceramide-treated snc1^ala43 cells shifted to restrictive temperatures. snc cells expressing snc1^ala43 (JG8-SNC1A43L) were grown in glucose-containing medium at 26°C and either maintained at 26°C during labeling or shifted for 0.5 h to 37°C, before labeling with FM4-64 at the restrictive temperature. Some cells were treated with C₂-ceramide (+C₂) during growth at 26°C.

Similarly, we found that the mutation of VBM1 in snc tlg cells also restored FM4-64 staining of the vacuole as well as conferringnormal vacuole biogenesis (Figure 1B). Thus, both ceramide treatmentand vbm mutation have identical effects. Finally, we tested whetherceramide treatment could restore vacuolar staining in temperature-shiftedsnc1^ala43 cells (Figure 1C). Indeed, we found that staining of vacuoleswas normal in snc1^ala43 cells shifted to 37°C for 2 h. Therefore, defects that arisefrom inactivating mutations in the v- and t-SNAREs involved inendocytosis are corrected upon CAPPactivation.

Because ceramide treatment or vbm mutation result in the dephosphorylation of Sso and rescue snc and sso2-1 cells (Marashand Gerst, 2001), it was possible that the enhanced rate of exocytosisalone might confer an improvement in endocytosis. To test this,we expressed a constitutively activated form of Sso1 (Sso1^ala79; Marash and Gerst, 2001), which rescues snc cells in the absenceof CAPP activation, in snc yeast and examined the uptake of FM4-64.In contrast to ceramide-treated cells, FM4-64 was unable to labelvacuoles or vacuolar bodies in snc yeast expressing Sso1^ala79, and the labeling was identical to that seen in control snc cells(Figure 2A). Thus, the effects of ceramide or vbm mutation onendocytosis are direct and not a result of enhanced exocytosis.

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Figure 2. SIT4, but not SSO1^ala79, overexpression restores the delivery of FM4-64 to the vacuole in snc cells. (A) Expression of SSO1^ala79 does not restore FM4-64 labeling of the vacuole. snc yeast (JG8) transformed with a plasmid expressing SSO1^ala79 were grown on galactose-containing medium at 26°C, before being shifted to glucose-containing medium for 36 h to deplete Snc1. Cells were incubated with FM4-64 at 26°C and processed for microscopy. (B) SIT4 overexpression restores FM4-64 labeling of the vacuole. snc cells (JG8) transformed with a plasmid expressing SIT4 were grown and labeled with FM4-64 as described above. (C) Ceramine treatment and SIT4 overexpression restore FM4-64 labeling of the vacuole in tlg yeast. tlg1 and tlg2 yeast treated with (+C₂) or without ( $-$ C₂) ceramide, or overexpressing SIT4, were labeled with FM4-64 and processed for microscopy.

Overproduction of Sit4 Confers FM4-64 Labeling of the Vacuole in snc and tlg Null Cells

Rescue of growth and exocytosis in snc cells by either ceramide treatment or vbm mutation necessitates the activation of thecatalytic subunit of CAPP, Sit4 (Nickels and Broach, 1996), whoseoverexpression can also rescue snc yeast (Marash and Gerst, 2001).Therefore, we next examined whether SIT4 overexpression alonecould confer the normal uptake of FM4-64 to thevacuole.

We found that snc cells transformed a plasmid expressing SIT4 gave normal staining of the vacuole by FM4-64, after being shiftedfrom galactose-containing medium to glucose-containing medium(Figure 2B). This rescue was apparent up to 36 h after the shift.However, at later time points it also became apparent that thisrestoration was temporal, because hazy staining of the cytoplasmand vacuolar fragmentation became more obvious (our unpublishedresults). This time-dependent decrease in the ability of SIT4overexpression to restore FM4-64 trafficking could be reversedupon the addition of ceramide into the medium (our unpublishedresults).

Finally, we examined whether ceramide addition or SIT4 overexpression could confer normal FM4-64 staining of the vacuole intlg1 and tlg2 mutant cells (Figure 2C). As shown above for sncand snc tlg cells, defects in FM4-64 labeling of the vacuole intlg cells were abolished upon ceramide addition or SIT4overexpression.

Ligand-mediated Delivery of the Ste2 Mating Factor Receptor to the Vacuole Is Restored in snc, snc tlg, and Temperature-shifted snc1^ala43 Cells by Ceramide Addition or vbm Mutation

Because defects in FM4-64 delivery to the vacuole in snc and tlg mutant yeast are restored independently by CAPP activation,we examined whether ligand-mediated uptake of a cell surface receptoris also rescued. Previously, we demonstrated that uptake of aSte2-GFP fusion protein (Stefan and Blumer, 1999) to the vacuole(after $alpha$ -factor treatment) was blocked in snc and temperature-shiftedsnc1^ala43 cells (Gurunathan et al., 2000).

In snc cells (JG8) shifted to glucose-containing medium for 36 h, we found both Ste2-GFP and Ste2-tailGFP present primarilyon the plasma membrane in both untreated and $alpha$ -factor-treatedcells (Figure 3A), as described previously. The Ste2-tail GFPprotein is deficient in its ability to be endocytosed (Stefanand Blumer, 1999) and served as a control. In contrast to thesnc control cells, snc cells expressing SNC1 showed a time-dependentuptake of Ste2-GFP upon $alpha$ -factor treatment, as described (Gurunathanet al., 2000). We then checked whether ceramide addition had aneffect on Ste2 uptake in $alpha$ -factor-treated snc yeast. Additionof ceramide restored the time-dependent uptake of Ste2-GFP, butnot of Ste2-tailGFP, to the vacuole (Figure 3A). The disappearanceof Ste2-GFP in ceramide-treated snc cells was similar to thatseen for snc cells expressing SNC1, upon $alpha$ -factor addition. Thus,ceramide treatment restored endocytic uptake of a membrane proteinin snc cells.

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Figure 3. Ligand-mediated delivery of Ste2 to the vacuole is restored in snc, snc tlg, and temperature-shifted snc1^ala43 cells by CAPP activation. (A) Delivery of Ste2-GFP, but not Ste2-tailGFP, to the vacuole is restored in ceramide-treated snc cells. snc cells (JG8) expressing either Ste2-GFP (snc STE2GFP) or a truncated form of Ste2-GFP (snc STE2-tailGFP), which does not undergo endocytosis, were grown to log phase in galactose-containing medium at 26°C, before being shifted to glucose-containing medium with (+C₂) or without ( $-$ C₂) added C₂-ceramide (10 µM) for 36 h, and before labeling with FM4-64. After labeling, cultures were split, whereby half was mounted in soft agar containing no additions, whereas the other half was mounted in agar containing $alpha$ -factor (1 µM) and processed immediately for microscopy. snc cells expressing SNC1 constitutively (SNC1 STE2GFP) were used as control. Cells were monitored by confocal microscopy as a function of time. Separate untreated cells (untreated) were used as controls. (B) Delivery of Ste2-GFP to the vacuole is restored in ceramide-treated snc tlg cells. snc tlg1 (JG9-TLG1) and snc tlg2 cells (JG9-TLG2) expressing Ste2-GFP (snc tlg1 STE2GFP or snc tlg2 STE2GFP) from the kan^r plasmid were grown in galactose-containing medium at 26°C, before being shifted to glucose-containing medium with (+C₂) or without ( $-$ C₂) C₂-ceramide (10 µM). After 24 h, cells were labeled with FM4-64, treated with $alpha$ -factor and processed for microscopy. (C) Ligand-mediated delivery of Ste2-GFP to the vacuole is restored in snc cells bearing a mutation in VBM1. snc vbm1 cells (MM1) expressing either Ste2-GFP (snc vbm1 STE2GFP) or the truncated form of Ste2-GFP (snc vbm1 STE2-tailGFP) were grown to log phase at 26°C in glucose-containing medium, before labeling with FM4-64, treatment with $alpha$ -factor, and processing for microscopy. (D) Ligand-mediated delivery of Ste2-GFP to the vacuole occurs in temperature-shifted snc1^ala43 cells upon ceramide treatment. snc1^ala43 cells (JG8-SNC1A43L) expressing Ste2-GFP were grown at 26°C in glucose-containing medium with (+C₂) or without ( $-$ C₂) C₂-ceramide (10 µM). Half of each culture was shifted to prewarmed medium (37°C), for 1 h before FM4-64 labeling and treatment with $alpha$ -factor at the restrictive temperature.

Because ceramide treatment restored FM4-64 labeling of the vacuole in snc tlg cells, we examined the uptake of Ste2-GFP inthese strains (Figure 3B). As can be seen, ceramide-treated snctlg1 and snc tlg2 cells responded to $alpha$ -factor addition and Ste2-GFPwas delivered to the vacuole in a time-dependent manner. In contrast,no change in Ste2-GFP localization was observed in untreated cells,after $alpha$ -factor addition. Thus, ceramide treatment restores Ste2uptake in cells lacking one of the TLG genes as well as in cellslacking both SNCgenes.

Next, we examined whether Ste2-GFP uptake in snc cells is restored by vbm mutation. We measured Ste2-GFP uptake after $alpha$ -factoraddition to snc vbm1 cells (Figure 3C). As expected Ste2-GFP,but not Ste2-tailGFP, was delivered to the vacuole as shown abovefor ceramide-treated snc cells or snc cells expressing SNC1 (Figure3, A andB).

Finally, we examined the uptake of Ste2-GFP in snc1^ala43 cells that were shifted to the restrictive temperature (37°C), beforethe addition of $alpha$ -factor (Figure 3D). We found that Ste2-GFP wasdelivered to the vacuole in ceramide-treated, but not untreated,snc1^ala43 cells at 37°C. In contrast, Ste2-GFP was taken up in the absenceof ceramide at 26°C. Thus, ceramide treatment can confer the uptakeand delivery of Ste2 to the vacuole in snc, snc tlg, and in temperature-shiftedsnc1^ala43cells.

Ste2 Is Degraded in Ceramide-treated snc and Temperature-shifted snc1^ala43 Cells

In yeast, some membrane proteins undergo ubiquitin-dependent endocytosis that delivers the internalized protein to the vacuolefor degradation (Hicke, 1999). To verify that Ste2 is degradedin ceramide-treated snc and snc1^ala43cells, as predicted by the experiments shown in Figure 3, we usedan HA-tagged form Ste2 (Ste2HA) in pulse-chase labeling experiments.Previously, we demonstrated that Ste2HA is stable for extendedperiods in its higher molecular weight, presumably ubiquitinated/phosphorylatedform, in $alpha$ -factor-treated snc and temperature-shifted snc1^ala43 cells (Gurunathan et al., 2000). We next tested whether ceramidetreatment could restore the normal degradation of Ste2HA in thesecells after $alpha$ -factor treatment (Figure 4).

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Figure 4. Ceramide treatment restores the degradation of Ste2 in snc and temperature-shifted snc1^ala43 cells. snc (JG8) and snc1^ala43 (JG8-SNC1A43) cells expressing Ste2HA were grown to log phase in glucose-containing medium at 26°C with (+C₂) or without ( $-$ C₂) C₂-ceramide. snc cells expressing SNC1 constitutively (SNC1) were grown without ceramide and were used as control. Cells were pulse-labeled with [³⁵S]methionine and chased for 30 min in medium containing 5 mM methionine/cysteine, before treatment with $alpha$ -factor (1 µM). For snc1^ala43 cells, half of the cultures were shifted to prewarmed medium (37°C) for 1 h before labeling. At various times after treatment with $alpha$ -factor (2-60 min), samples were removed, extracts were prepared, and Ste2HA was IP'd using anti-HA antibodies. Ste2HA was detected by autoradiography.

We found that Ste2HA is stable for up to 60 min in $alpha$ -factor-treated snc and temperature-shifted snc1^ala43 cells that were not treated with ceramide (Figure 4), as wasshown previously. Both the lower (47 kDa) and higher (54 kDa)molecular weight forms were apparent, the lower form being presentbefore $alpha$ -factor addition. In contrast, C₂-ceramide treatment restoredthe degradation of Ste2 in both cell types (Figure 4). The highermolecular weight form apparent after 2 min was found to disappearbetween 20 and 40 min after the addition of $alpha$ -factor. The rateof degradation was similar to that seen in snc yeast expressingSNC1. Thus, as suggested by the GFP fluorescence data (Figure3), ceramide treatment restores Ste2 degradation in snc and temperature-shiftedsnc1^ala43 cells upon $alpha$ -factoraddition.

Ceramide Treatment Enhances Tlg Assembly into Complexes in snc and snc tlg Cells

Our results show that CAPP activation normalizes both the exocytic (Marash and Gerst, 2001) and endocytic pathways (this study).Previously, we demonstrated that rescue of the exocytic path dependson dephosphorylation of the Sso1,2 t-SNAREs, which assemble intot-t-SNARE complexes with Sec9 to, presumably, form the functionaltrans complex (Marash and Gerst, 2001). The question arises asto which t-SNAREs mediate the endocytosis of materials from thecell surface and whether they also undergo Sit4-dependentdephosphorylation.

Physical and genetic studies show that the Tlg t-SNAREs are involved in endocytosis and interact with the Snc v-SNAREs (Abeliovichet al., 1998; Holthuis et al., 1998a; Seron et al., 1998; Groteand Novick, 1999; Gurunathan et al., 2000). Thus, it is likelythat Tlg2, a syntaxin-like t-SNARE, and Tlg1, a SNARE light-chain,form complexes with Snc1,2 at endosomes or the trans-Golgi (TGN).Although Tlg2 has been proposed to act at early endosomes (Abeliovichet al., 1998; Seron et al., 1998), it overlaps with Tlg1, whoseplacement is broader and encompasses the TGN (Holthuis et al.,1998a, 1998b; Coe et al., 1999). Thus, we conjectured that Tlg1and 2 could be partners, along with Snc1 or Snc2, in SNARE complexesrelevant to endocytic functioning. Although not the focus of thiswork, a fourth helix is probably contributed to the complex byother SNAREs involved in endosomal functioning, i.e.,Vti1.

Both Tlg1 and Tlg2 are phosphorylated in vivo (our unpublished results); thus, we examined whether these t-SNAREs are presentin complexes in snc cells and whether the amounts of these complexesincrease upon ceramide treatment. By performing coimmunoprecipitation(coIP) experiments, we found that Tlg1 precipitates from snc celllysates with anti-Tlg2 antibodies and that the amount of Tlg1in a complex with Tlg2 goes up by substantially after ceramidetreatment (Figure 5A). Thus, the assembly of Tlg1 and 2 into SNAREcomplexes is modulated by CAPP activation. Next, we performeda complimentary experiment whereby we examined whether PKA overexpressionaffects the assembly of Tlg1 and Tlg2 into complexes in wild-typecells. We found that TPK1 overexpression lowered the amount ofTlg1 and Tlg2 present in complexes by half (Figure 5B). Thus,both the CAPP and PKA signaling paths modulate Tlg SNARE assemblyin vivo.

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Figure 5. Ceramide treatment promotes Tlg assembly into Tlg-Tlg SNARE complexes in vivo, whereas Tlg phosphorylation by Tpk1 inhibits assembly in vitro and in vivo. (A) C₂-ceramide treatment promotes Tlg1-Tlg2 complex assembly in snc cells. snc cells (JG8) were grown to log phase with (+C₂) or without C₂-ceramide ( $-$ C₂; 10 µM). Cell extracts were prepared and Tlg1-Tlg2 SNARE complexes were IP'd using purified anti-Tlg2 antibodies (abs) and detected using either anti-Tlg1 or anti-Tlg2 abs. TCL, total cell lysate (100 µg protein/lane). A histogram of the IP data, after normalization for the expression of TLG1 and TLG2, and subtraction of the background, is shown. Density is given in arbitrary units. (B) TPK1 overexpression inhibits the assembly of Tlg1 and Tlg2 in wild-type cells. Lysates were prepared from SP1 cells that either expressed TPK1 (+TPK1) or not ( $-$ TPK1) and had been treated either with (+C₂) or without C₂-ceramide ( $-$ C₂). Tlg1-Tlg2 complexes were IP'd using anti-Tlg2 abs, and Tlg1 was detected in immunoblots using anti-Tlg1 abs. Data are represented in histograms, as described in A. (C) Ceramide treatment promotes formation of a Tlg1-Tlg1 complex in snc tlg2 cells. snc tlg2 cells expressing myc-Tlg1 were grown to log phase with (+C₂) or without C₂-ceramide ( $-$ C₂; 10 µM). Cell extracts were prepared and myc-Tlg1 was IP'd using anti-myc abs and detected using anti-Tlg1 abs. TCL, total cell lysate (100 µg protein/lane); IP, immunoprecipitate. Data are represented in histograms, as described in A. (D) Ceramide treatment promotes formation of a Tlg2-Tlg2 complex in snc tlg1 cells. snc tlg1 cells expressing myc-Tlg2 were grown to log phase with (+C₂) or without C₂-ceramide ( $-$ C₂; 10 µM). Cell extracts were prepared and myc-Tlg2 was IP'd using anti-myc abs and detected using anti-Tlg2 abs. TCL, total cell lysate (100 µg protein/lane); IP, immunoprecipitate. Data are represented in histograms, as described in A. (E) In vitro phosphorylation of GST-Tlg1^1-206 and GST-Tlg2^1-317 by Tpk1 and dephosphorylation by Sit4. GST-Tlg1^1-206 and GST-Tlg2^1-317 were phosphorylated in vitro using Tpk1 and radiolabeled ATP for 1 h at 30°C with or without added Sit4 or Sit4 and C₂-ceramide. Proteins were resolved on SDS-PAGE gels and detected by autoradiography or by staining with Coomassie blue. A histogram of the autoradiography data is shown. (F) Tlg-Tlg assembly is inhibited by phosphorylation. Recombinant GST-Tlg1^1-206 and GST-Tlg2^1-317 were phosphorylated in vitro using recombinant Tpk1 and ATP. After phosphorylation, the proteins were mixed and IP'd using anti-Tlg1 abs. In parallel, unphosphorylated GST-Tlg1^1-206 and GST-Tlg2^1-317 were also mixed and IP'd using anti-Tlg1 abs. GST-Tlg2^1-317 that coIP'd with GST-Tlg1^1-206 was detected using anti-Tlg2 abs. Data are represented in a histogram, as described in A.

Interestingly, CAPP activation did not block the effect of TPK1 overexpression in wild-type cells (Figure 5B) and did notincrease Tlg assembly in snc cells expressing SNC1 (our unpublishedresults). This suggests that the A kinase signaling pathway hasa dominant effect in the wild-type background. We also examinedwhether expression of the activated form of Sso1 (Sso1^ala79) affects Tlg1-Tlg2 assembly in snc cells; however, we found noincrease in the level of complex formation (our unpublished results).Thus, an enhancement in exocytosis, as mediated by Sso1^ala79, does not influence Tlg SNARE assembly (our unpublished results)or endocytosis per se (Figure 2A).

Because CAPP activation confers endocytosis to snc tlg and tlg cells, which lack one of the Tlg proteins, we examined whetherceramide treatment increases assembly of the remaining Tlg intomultimeric complexes. This phenomenon was observed previouslywith the Sso t-SNAREs after ceramide treatment (Marash and Gerst,2001). We found that ceramide treatment increased the coIP ofnative Tlg1 with myc-Tlg1 by about twofold in lysates preparedfrom snc tlg2 cells that express a myc epitope-tagged form ofTlg1 (Figure 5C). Likewise, ceramide treatment increased the coIPof native Tlg2 with myc-Tlg2 by twofold in lysates prepared fromsnc tlg1 cells expressing myc-Tlg2 (Figure 5D). Thus, individualTlg t-SNAREs multimerize in response to CAPP activation and, presumably,dephosphorylation.

Tlg Phosphorylation In Vitro by Tpk1 Inhibits Assembly into Complexes

To examine whether Tlg phosphorylation also inhibits assembly in vitro, we expressed recombinant Tlg1 and Tlg2 (lacking theirmembrane-spanning domains) as GST-fusion proteins in bacteria.Affinity-purified proteins were phosphorylated in vitro with Tpk1(Marash and Gerst, 2001) and used in subsequent binding reactions.Both recombinant Tlg1 and Tlg2 underwent Tpk1-dependent phosphorylationas well as Sit4-dependent dephosphorylation (Figure 5E). The latterwas markedly enhanced by the addition of C₂-ceramide into theassay mixture. Binding assays using either phosphorylated or unphosphorylatedproteins revealed that the unphosphorylated Tlg t-SNAREs formedtwo- or threefold more heteromeric complexes than the phosphorylatedproteins (Figure 5F). Thus, these endosomal t-SNAREs appear toundergo the same types of regulation shown for the Sso exocytict-SNAREs, both in vivo and in vitro (Marash and Gerst, 2001).

Mutations in Putative PKA Sites in Tlg1 and 2 Result in Activated t-SNAREs that Confer Endocytosis, but not Exocytosis in snc Cells

Because the restoration of endocytosis by CAPP activation correlates with Tlg dephosphorylation and assembly, we examinedpotential sites for phosphorylation in Tlg1 and Tlg2. As shownpreviously (Marash and Gerst, 2001), mutation of a PKA site (ser-79)in the autoinhibitory domain (Habc) of Sso confers full exocyticfunctioning in the absence of CAPP activation. Therefore, we mutatedputative PKA sites in the same region of Tlg1 (e.g., thr-31) andTlg2 (e.g., thr-6, -15, -54, -138, and ser-90, -101) by site-directedmutagenesis. We tested these mutants for their ability to conferthe uptake of FM4-64 in snc yeast in the absence of CAPP activation(Figure 6A and our unpublished results). We found that alaninesubstitutions at position 31 of Tlg1 and position 90 of Tlg2 restoredFM4-64 uptake to the vacuole in snc cells (Figure 6A). In contrast,the other alanine substitutions in Tlg2 were unable to do so (ourunpublished results).

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Figure 6. Mutation of thr-31 in Tlg1 and ser-90 in Tlg2 is sufficient to restore endocytosis, but not exocytosis, to snc yeast. (A) Mutation of thr-31 in Tlg1 and ser-90 in Tlg2 restores endocytosis to snc yeast. snc cells (JG8) expressing a control plasmid (snc) or overexpressing SNC1, TLG1, TLG2, TLG1^ala31, or TLG2^ala90 were grown, shifted to glucose-containing medium for 24 h, and labeled with FM4-64. Cells were visualized using Nomarski optics (Light) or via the rhodamine channel (FM4-64). (B) Mutation of thr-31 in Tlg1 and ser-90 in Tlg2 does not restore growth to snc yeast. snc cells (JG8) expressing a control plasmid (snc) or overexpressing SNC1, TLG1^ala31, TLG2^ala90, SSO1^ala79, or both SSO1^ala79and TLG1^ala31 or SSO1^ala79 and TLG2^ala90 were grown, shifted to glucose-containing medium for 24 h, diluted serially and plated onto galactose-containing medium (SC+GAL) at 26°C, glucose-containing medium (SC+GLU) at 26, 35.5, or 37°C, or amino acid-rich medium (YPD) at 26°C. Cells were grown for 48 h.

When tested for conferring growth to snc cells, we found that expression of these mutant Tlg proteins had no significant effectalone, but did enhance the rescue mediated by Sso1^ala79 (Figure 6B). Thus, the presence of Sso1^ala79 and Tlg1^ala31 or Sso1^ala79 and Tlg2^ala90 restored normal growth (exocytosis) and endocytosis in the absenceof CAPP activation. Moreover, their growth appeared more robustthan that of snc cells expressing SNC1. Thus, abolishment of thesePKA sites leads to dominant effects on the exo- and endocyticpathways in sncyeast.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Earlier we demonstrated that yeast lacking the SNC genes (snc, snc tlg1, and snc tlg2 cells) or bearing a temperature-sensitiveallele of SNC1 (snc1^ala43, snc1^ala4tlg1, and snc1^ala4 tlg2 cells) are deficient in the endocytic uptake of componentsfrom the cell surface (Gurunathan et al., 2000). Thus, the Sncexocytic v-SNAREs are actively involved in endocytosis. More recentwork suggests that CAPP activation allows snc and sso2-1 cellsto overcome blocks in exocytosis, via dephosphorylation of theSso t-SNAREs and their subsequent assembly into SNARE complexeswith Sec9 (Marash and Gerst, 2001). Thus, we examined whetherthe endocytic defects present in snc and snc tlg cells are alsoameliorated upon CAPP activation. Our results show that ceramidetreatment, VBM inactivation, or SIT4 overexpression (all of whichlead to CAPP activation) confer normal endocytic functioning toyeast lacking the endocytic v-SNAREs (snc cells), endocytic t-SNAREs(tlg1 and tlg2 cells), or both (snc tlg1 and snc tlg2 cells; Figures1-3). We had expected snc tlg cells to be even more inhibited inendocytic functions than snc cells, because of the loss of anadditional component of the endocytic fusion complex. Nevertheless,CAPP activation also rescues these triple mutants. Thus, CAPPhas a prominent role in the control of endocytic functions aswell as exocytic functions, as described previously (Marash andGerst, 2001).

The restoration of endocytosis also involves t-SNARE dephosphorylation and assembly, as ceramide-treated snc cells showeda large increase in Tlg1-Tlg2 complex formation (Figure 5A), whereassnc tlg1 and snc tlg2 cells showed an increase in the formationof Tlg2-Tlg2 or Tlg1-Tlg1 complexes, respectively (Figures 5,C and D). Correspondingly, recombinant Tlg t-SNAREs phosphorylatedin vitro showed a reduced ability to assemble into complexes (Figure5F). Thus, phosphorylation appears to modulate Tlg SNARE assembly,as shown previously for the Sso t-SNAREs (Marash and Gerst, 2001).Interestingly, endocytosis could be restored completely in snccells expressing mutant Tlg proteins that bear alanine substitutionsin specific PKA phosphorylation sites (Figure 6A). Thus, the Tlgendosomal t-SNAREs are likely receivers of regulatory signalsarising from the PKA and CAPP pathways, as shown previously forthe Sso1,2 exocytic t-SNAREs (Marash and Gerst, 2001).

It is clear from our ongoing work that t-SNARE phosphorylation plays a prominent role in controlling SNARE assembly, particularlyin cells that have transport defects. Signaling via the Sit4 catalyticsubunit of CAPP relieves environmental stresses placed on thecell (Hannun and Luberto, 2000) as well as blocks in protein traffickingand cell growth (Marash and Gerst, 2001 and this study). Theseblocks can be at various points in the endo- and exocytic pathwaysand are modulated by PKA, which confers growth signals based onnutrient availability. Thus, signaling paths that inhibit thecell cycle in wild-type cells, such as the CAPP pathway, and thosethat stimulate entry, such as the RAS-adenylyl cyclase-PKA pathway,meet at the level of vesicle trafficking. The interactions betweenthese pathways, clearly evident in yeast secretion mutants, arealso likely to be operative in wild-type cells although the physiologicalbasis remains undefined. At this point we do not believe thatt-SNAREs undergo phosphorylation and dephosphorylation duringeach round of SNARE assembly, because alanine substitutions (whichprevent phosphorylation) in the relevant PKA sites of Sso andTlg actually enhance protein trafficking (Figure 6 and Marashand Gerst, 2001). It is more likely that phosphorylation regulatesthe availability of t-SNAREs to participate in trafficking events,although additional work is required to understand this importantmechanism.

Other groups have shown that sphingoid bases are involved in endocytosis. Zanolari et al. (2000) demonstrated that sphingoidbase synthesis is required for internalization in Saccharomycescerevisiae, as a lcb1 mutant (involved in serine palmitoyltranferaseactivity) is defective in endocytic uptake. Moreover, Grote etal. (2000) identified a phosphosphingosine lyase (Dlp1) as a multicopysuppressor of the snc phenotype. Overexpression of Dlp1 also rescuedendocytic defects resulting from the Snc1^ala43 protein at restrictive temperatures. From the mechanistic pointof view, it would appear that Dlp1 elevates the intracellularlevels of sphingosine, which we have shown to activate CAPP andlead to the dephosphorylation of Sso (Marash and Gerst, 2001)and Tlg (this study). Interestingly, Friant et al. (2000) demonstratedthat the inactivation of other PP2A catalytic subunits (includingPph21, Pph22, and Pph3, but not Sit4) abrogates the sphingoidbase requirement in endocytosis. However, these other PP2A subunitshad no effect on blocks in exocytosis and could not rescue snccells (Marash and Gerst, 2001). Thus, Sit4 alone regulates bothendo- and exocytosis, whereas the other PP2A catalytic subunitsact more specifically (and, apparently, in a contrary manner)at the endocytic level. Because Sit4 dephosphorylates t-SNAREsthat have been phosphorylated by PKA, it is likely that the otherPP2A activities modulate endocytosis in a differentmanner.

Ceramides also act as regulators of intracellular trafficking events in mammalian cells (Hannun and Luberto, 2000). For example,the production of ceramide by sphingomyelinase elicits phagocytosis(Grassme et al., 1997; Hinkovska-Galcheva et al., 1998; Zha etal., 1998). Likewise, ceramide treatment has been shown to inducethe formation of endocytic vesicles (Li et al., 1999). Thus, itis possible that mammalian CAPP acts on protein trafficking ina similar manner as shown foryeast.

Another finding to come from this work is that ceramide treatment bypasses the deletion of either TLG gene and confers endocytosis.Thus, the rescue mechanism by which CAPP acts is operative inthe absence of the endosomal v- or t-SNAREs alone, or in combination.Deletion of either TLG gene is known to affect intracellular proteintrafficking and endocytic functions to a degree and in some celltypes leads to lethality (Coe et al., 1999), although conditionallethal strains bearing deletions in both genes have been reported(Holthuis et al., 1998a). In our strain background, TLG deletionshave prominent effects on endocytosis, but only small effectson cell growth (Gurunathan et al., 2000). Based on the work shownhere, it is likely that the deletion of individual TLG genes istolerated in snc cells, perhaps because of the ability of Tlgproteins to form homomeric complexes (Figure 5, C and D). Althoughthis, by itself, is insufficient to confer endocytosis, CAPP activationby ceramide treatment, VBM/ELO inactivation, or SIT4 overexpression,clearly overcomes any inhibition placed on the existing Tlg t-SNARE.This inhibition is likely to result from Tlg phosphorylation byPKA, based on the in vitro and in vivo experiments performed here(Figures 5 and 6). Thus, as shown earlier for the Sso t-SNAREs(Marash and Gerst, 2001), phosphorylation of the Tlg t-SNAREsmodulates their ability to confer endocytic trafficking by inhibitingSNARE assembly. Although the constituents of the endocytic SNAREcomplex have not been completely resolved, combinations involvingTlg1 and Tlg2 with the Snc v-SNAREs as well as other endosomalSNAREs (i.e., Vti1) are likely to occur. Very recently, two studiesdemonstrated that Tlg1 and 2 assemble into complexes along withVti1 to mediate the fusion of trans-Golgi membranes and liposomesin vitro (Brickner et al., 2001; Paumet et al., 2001). Moreover,liposome fusion was dependent on the presence of a Snc v-SNARE,suggesting that a Tlg1-Tlg2-Vti1-Snc complex mediates endosomaltrafficking (Paumet et al., 2001). Whether this complex formsin wild-type yeast in vivo has yet to be determined. Moreover,the constituents of the SNARE complexes formed in the two snctlg strains (which become competent for endocytosis upon CAPPactivation) are unknown. Perhaps, a functional t-t-SNARE complex,like that proposed to exist at the exocytic level (Marash andGerst, 2001), can also confer endocytosis in the absence of theSnc v-SNAREs.

	ACKNOWLEDGMENTS

The authors thank Hagai Abeliovich, Kendall Blumer, Hugh Pelham, and Michael Wigler for the generous gifts of antibodies andreagents and Vera Shindler for electron microscopy. This workwas generously supported by a grant from the Minerva Foundation,Germany. J.E.G. holds the Henry Kaplan Chair in CancerResearch.

	FOOTNOTES

^* Corresponding author. E-mail address: jeffrey.gerst{at}weizmann.ac.il.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.01-11-0541. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.01-11-0541.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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