Synthetic Genetic Array Analysis of the PtdIns 4-kinase Pik1p Identifies Components in a Golgi-specific Ypt31/rab-GTPase Signaling Pathway

Vicki A. Sciorra^*, Anjon Audhya^*, Ainslie B. Parsons, Nava Segev, Charles Boone, and Scott D. Emr^*

^* Department of Cellular and Molecular Medicine and the Howard Hughes Medical Institute, School of Medicine, University of California at San Diego, La Jolla, CA 92093-0668; Banting and Best Department of Medical Research and Department of Medical Genetics and Microbiology, University of Toronto, Toronto, Ontario, Canada M5G 1L6; and Department of Biological Sciences, Laboratory for Molecular Biology, University of Illinois at Chicago, Chicago, IL 60607

Submitted August 13, 2004; Accepted November 19, 2004
Monitoring Editor: Randy Schekman

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Phosphorylated derivatives of phosphatidylinositol are essentialregulators of both endocytic and exocytic trafficking in eukaryoticcells. In Saccharomyces cerevisiae, the phosphatidylinositol4-kinase, Pik1p generates a distinct pool of PtdIns(4)P thatis required for normal Golgi structure and secretory function.Here, we utilize a synthetic genetic array analysis of a conditionalpik1 mutant to identify candidate components of the Pik1p/PtdIns(4)Psignaling pathway at the Golgi. Our data suggest a mechanisticinvolvement for Pik1p with a specific subset of Golgi-associatedproteins, including the Ypt31p rab-GTPase and the TRAPPII proteincomplex, to regulate protein trafficking through the secretorypathway. We further demonstrate that TRAPPII specifically functionsin a Ypt31p-dependent pathway and identify Gyp2p as the firstbiologically relevant GTPase activating protein for Ypt31p.We propose that multiple stage-specific signals, which may includePik1p/PtdIns(4)P, TRAPPII and Gyp2p, impinge upon Ypt31 signalingto regulate Golgi secretory function.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The Golgi apparatus plays an essential role in the intracellulartrafficking and sorting of proteins and lipids within the secretorypathway. Although the Golgi complex in mammalian and yeast cellsare morphologically different, they are both organized intofunctionally distinct compartments: the cis-, medial- and trans-Golgi(Franzusoff and Schekman, 1989; Graham and Emr, 1991). EachGolgi compartment has a unique repertoire of resident proteinsthat are responsible for the sequential posttranslational modificationand maturation of cargo proteins, which are then secreted outof the Golgi and transported to their cellular destinations(i.e., to the plasma membrane, endosome, or lysosome/vacuole).Transport to and from the Golgi requires the concerted actionsof specific rab-GTPases, SNAREs, phosphoinositides, and hetero-oligomericprotein complexes (Segev, 2001; Zerial and McBride, 2001; Pfeffer,2003). The coordinated action of these diverse transport componentsprovides specificity in each trafficking step, although themechanism by which these components cooperate in Golgi traffickingis only partially understood.

Phosphorylated derivatives of phosphatidylinositol are particularlyversatile regulators of protein transport and carry out essentialmodulatory functions within the secretory pathway by interactingwith distinct lipid-binding effector molecules (Simonsen etal., 2001). For instance, phosphatidylinositol 3-phosphate (PtdIns(3)P)is required for the anterograde traffic of cargo proteins fromthe Golgi to the vacuole by interacting with specific proteinsthat contain either a FYVE domain or a Phox homology (PX) domain,two motifs which specifically bind PtdIns(3)P (Simonsen et al.,2001). Conversely, phosphatidylinositol 4-phosphate (PtdIns(4)P),regulates the traffic of cargo proteins from the Golgi to theplasma membrane (Hama et al., 1999; Walch-Solimena and Novick,1999; Audhya et al., 2000) by a yet undefined mechanism.

Saccharomyces cerevisiae contains two essential phosphatidylinositol4-kinases, Stt4p and Pik1p. Functional studies have demonstratedthat Pik1p and Stt4p catalyze the production of the majorityof PtdIns(4)P in yeast (Audhya et al., 2000) and suggest uniqueroles for the two pools of PtdIns(4)P synthesized by each PtdIns4-kinase. In part this is due to the differential subcellulartargeting of Stt4p and Pik1p. Stt4p localizes to the cell periphery(Audhya and Emr, 2002) and regulates cell wall integrity andvacuole morphology but has no detected role in secretion (Audhyaet al., 2000). In contrast, Pik1p localizes to both the Golgi(Walch-Solimena and Novick, 1999) and the nucleus (Garcia-Bustoset al., 1994; Walch-Solimena and Novick, 1999). Inactivationof Pik1p decreases PtdIns(4)P levels, impairs secretory transportfrom the Golgi, and disrupts the structural integrity of theGolgi and vacuole (Hama et al., 1999; Walch-Solimena and Novick,1999; Audhya et al., 2000). In addition, defects in cytokinesisand actin cytoskeletal organization have been observed afterloss of Pik1p function (Garcia-Bustos et al., 1994; Walch-Solimenaand Novick, 1999). Consequently, the pleiotropic effects causedby the inactivation of Pik1p have obscured the precise functionof PtdIns(4)P at the Golgi.

Mammalian cells express at least three Golgi-localized PtdIns4-kinases, PI4KII ${alpha}$ (Wang et al., 2003), PI4KIII ${alpha}$ (Nakagawa etal., 1996), and PI4KIII ${beta}$ (Wong et al., 1997). Subsequent studieshave found that PI4KIII ${beta}$ is recruited to the Golgi by active,GTP-bound Arf (Godi et al., 1999). Interfering with PI4KIII ${beta}$ by the overexpression of a kinase dead, dominant-negative mutant,disrupted the structural integrity of the Golgi (Godi et al.,1999), providing additional evidence for PtdIns(4)P in the regulationof Golgi function. Arf also recruited an unidentified PtdIns(4)P5-kinase to the Golgi, resulting in the conversion of PtdIns(4)Pto PtdIns(4,5)P₂, making the respective roles of PtdIns(4)Pand PtdIns(4,5)P₂ at the Golgi less clear (Godi et al., 1999).Inactivation of temperature-sensitive alleles of MSS4, the solephosphoinositide kinase responsible for the synthesis of PtdIns(4,5)P₂in yeast, does not affect the morphology or secretory functionof the Golgi complex (Audhya and Emr, 2002; Stefan et al., 2002).Collectively, these data suggest that PtdIns(4)P serves multiplefunctions, as a direct mediator in Golgi function, and as aprecursor to PtdIns(4,5)P₂.

To gain a better understanding of the essential role of Pik1pin yeast Golgi function, we have utilized a synthetic geneticarray (SGA) analysis to identify genes that may participatein a Pik1p-dependent pathway. We report the identification ofPIK-specific genetic interactions with genes known to have distinctroles in membrane trafficking and Golgi function. We demonstratethat Pik1p functionally interacts with Ypt31p, a Golgi-localizedrab-GTPase, to regulate the trafficking of cargoes that requirerecycling through the early endosome, including the yeast SNARE,Snc1p, and chitin synthase, Chs3p. Using information obtainedfrom the screen, we present evidence that transport proteinparticle (TRAPP) complex II, a large protein complex localizedto the Golgi (Sacher et al., 2001), interacts genetically withPIK1 and functionally with Ypt31p. Further analysis of the interactionsbetween TRAPPII and Ypt31p led to the identification of Gyp2pas a biologically relevant GTPase activating protein (GAP) forYpt31p in vivo. Our comprehensive genetic analysis of the pik1mutation led to the dissection of relevant PtdIns(4)P-dependentpathways and to defining regulatory components that functionin Ypt31p rab-GTPase signaling at the Golgi.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Strains and Media
The genotypes of S. cerevisiae strains used in this study arelisted in Table 1. All yeast strains were grown in YPD or SDminimal media containing the necessary amino acid supplements.Transformations into yeast were performed by the lithium acetatemethod (Ito et al., 1983). All strains were constructed eitherby tetrad dissection of sporulated diploid strains or by integrationof indicated disruption cassettes as previously described (Longtineet al., 1998). Disruptions were confirmed by PCR. pik1-139^tsypt31 ${Delta}$ , pik1-139^ts kre11 ${Delta}$ ,and pik1-139^ts trs33 ${Delta}$ , and pik1–83^tsypt31 ${Delta}$ were isolated by tetrad dissection and maintained on YPD containing1 M sorbitol at 26°C. SEY6210 expressing TAT2-GFP or CHS3-GFPwere engineered by transformation of PCR-amplified genomic integrationconstruct using GFP-His3MX6 plasmid as template (Longtine etal., 1998) and verified by PCR analysis generating CJSY298 andVSY184. SEY6210 expressing GFP-SNC1 (VSY167) was engineeredby integrating an expression plasmid linearized with StuI atURA3 (Lewis et al., 2000) generating VSY167. pik1-139^ts, ypt31 ${Delta}$ and pik1-139^ts ypt31 ${Delta}$ double mutant cells expressing TAT2-GFP,CHS3-GFP, and GFP-SNC1 were isolated by tetrad dissection. Expressionof TAT2-GFP, CHS3-GFP, and GFP-SNC1 were screened by fluorescencemicroscopy and Western blotting.

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Table 1. S. cerevisiae strains used in this study

Genetic and DNA Manipulations
SGA analysis was performed as described previously (Tong etal., 2001). Standard molecular biology techniques were usedfor DNA manipulations (Maniatis et al., 1992). Enzymes usedfor recombinant DNA techniques were purchased from Roche (Nutley,NJ) and New England Biolabs (Beverly, MA). PCR reactions wereconducted as directed by manufacturer's instructions using PfuTurbo(Stratagene, La Jolla, CA) or AmpliTaq (Applied Biosystems,Foster City, CA) DNA polymerases for cloning and diagnosticreactions, respectively. Yeast genomic DNA was isolated by themethod of Hoffman and Winston (1987). A 1.8-kb fragment containingthe open reading frame (ORF) of YPT31 was amplified from genomicDNA prepared from SEY6210 using oligonucleotide primers thatincorporated unique BamHI and SmaI restriction enzyme sitesat the 5' and 3' ends, respectively. The PCR products were digestedwith BamHI and SmaI and subcloned into BamHI-SmaI–digestedpRS416 (Sikorski and Hieter, 1989) creating VSB283. Haploidypt31 ${Delta}$ and ypt32 ${Delta}$ single deletion mutants of opposite mating types,each expressing low-copy YPT31 were mated and sporulated andtetrads were isolated. ypt31 ${Delta}$ ypt32 ${Delta}$ double mutants carrying YPT31were confirmed by PCR and demonstrated functionality of theYPT31 clone. ypt31 Q72L (VSB333) and N126I (VSB334) were generatedby site-directed mutagenesis of the wild-type plasmid (VSB327)using the Quik-change kit (Stratagene) and confirmed by DNAsequencing. To generate GFP-YPT31, the YPT31 ORF (672 bp) wasamplified from pRS416-YPT31 engineered with BglII (5') and PstI(3') and subcloned into pGO37 (Burd and Emr, 1998) creatingVSB303. Expression of GFP-YPT31p was confirmed by Western blotanalysis. GFP-YPT31 was subsequently subcloned into NotI andSalI sites of pRS415 (Sikorski and Hieter, 1989) creating VSB311.ypt31 ${Delta}$ ypt32 ${Delta}$ double mutants carrying low copies of GFP-YPT31were isolated and confirmed as described above.

To generate a construct for expression of GFP-PIK1, a XhoI-KpnIfragment from pYcp50-PIK1, corresponding to the C-terminus ofPIK1, was first ligated into XhoI-KpnI–digested pGO36(Burd and Emr, 1998), creating pJA519. The N-terminus of PIK1with an 8-alanine linker and XhoI sites was amplified by PCRand cloned into XhoI-digested pJA519, creating pJA520 (GFP-PIK1).Expression of GFP-PIK1 in either pik1 ${Delta}$ or pik1^ts mutant cellsrescued lethality. To generate GFP-GYP2, the GYP2 ORF was amplifiedfrom genomic DNA prepared from SEY6210 using oligonucleotideprimers that incorporated unique EcoRI and ClaI restrictionenzyme sites at the 5' and 3', respectively. The PCR productwas digested with EcoRI and ClaI and ligated into EcoRI-ClaI–digestedpGO35 (Burd and Emr, 1998) creating VSB363. In frame GFP fusionswere confirmed by Western blot analysis. An NotI-ClaI fragmentcontaining GFP-GYP2 was subcloned into NotI-SmaI sites of pRS415(Sikorski and Hieter, 1989) creating VSB367. GFP-gyp2 G80E (VSB368)and GFP-gyp2 R295K (VSB369) were generated by site-directedmutagenesis, as described above.

A strain expressing the pik1-139^ts mutant plasmid was generatedin several steps. First, pRS415-PIK1 was linearized with NheI-NruI.Together with a randomly mutagenized PCR product correspondingto the C-terminal kinase domain of PIK1, these DNA fragmentswere transformed into pik1 ${Delta}$ ::HIS3 cells carrying pRS416-PIK1.Cells were incubated at 26°C and then transferred to platescontaining 5-FOA (to eliminate pRS416-PIK1) at both 26 and 37°C.Temperature-sensitive colonies were isolated, and individualplasmids were recovered. Temperature-sensitive alleles wereretested, and pik1-139 was chosen based on its ability to supportrobust growth of pik1 ${Delta}$ ::HIS3 cells at 26°C but not at temperaturesabove 35°C.

The ypt32 ${Delta}$ ypt31-101^ts temperature-sensitive mutant was generatedby a multistep process in which YPT31 (i.e., the entire YPT31ORF including a 200-base pair fragment downstream of the YPT31stop codon) was randomly mutagenized using AmpliTaq DNA polymeraseunder error-prone PCR conditions. URA3 was independently amplifiedunder nonerror prone PCR conditions. The mutagenized ypt31 andURA3 PCR fragments were cotransformed, fused to each other,and integrated into the YPT31 locus of ypt32 ${Delta}$ cells by homologousrecombination. Ura⁺ prototrophic transformants were selectedand screened for temperature-sensitive growth on YPD at 26 and38°C. A ypt32 ${Delta}$ strain harboring ypt31-101 (VSY468) displayedstrong temperature-sensitive phenotypes was selected for furthercharacterization.

pRC2240 SEC7-DsRED (Calero et al., 2003) was a gift from R.Collins (Cornell University). pHXT1-GFP (Malinska et al., 2003)was obtained from W. Tanner (Universitat Regensberg). pRS315-YPT6(Bensen et al., 2001) was obtained from G. Payne (UCLA) andthe 1.45-kb SacI-BamHI fragment from pRS315-YPT6 was subsequentlysubcloned into pRS425 (Sikorski and Hieter, 1989) creating VSB372.Plasmids for the expression of SEC4 and sec4 Q72L were giftsfrom P. Brenwald (UNC, Chapel Hill, NC). GFP-SNC1 integrationplasmid was from H. Pelham (MRC, United Kingdom).

Fluorescence and Electron Microscopy
Cells expressing GFP-PIK1 or GFP-YPT31 (or coexpressing SEC7-DsRED)were grown to early log phase at 26°C. After shifting to38°C for the indicated duration, cells were concentratedand visualized by fluorescence microscopy. Cells expressingGFP-SNC1, CHS3-GFP, TAT2-GFP, or HXT1-GFP were grown to earlylog phase and visualized at 26°C. Fluorescent images werevisualized using a Zeiss Axiovert S1002TV inverted fluorescentmicroscope (Thornwood, NY), acquired, and processed using aDelta Vision deconvolution system (Applied Precision Instruments,Issaquah, WA) and Adobe Photoshop 6.0 (San Jose, CA). Observationswere based on examination of at least 200 cells. Vacuole morphologywas examined by visualization of vacuole membranes by labelingwith the fluorescent dye, FM4–64 (Molecular Probes, Eugene,OR) as previously described by Vida and Emr (1995). For ultrastructuralanalysis, 50 OD₆₀₀ of early log-phase cells incubated at theappropriate temperature were harvested from YPD and fixed in3% glutaraldehyde, 0.1 M Na cacodylate (pH 7.4), 5 mM CaCl₂,5 mM MgCl₂, and 2.5% sucrose for 1 h. Cells were further processedfor electron microscopy as described previously (Audhya et al.,2000).

In Vivo Analysis of Phosphoinositides
Analysis of phosphoinositides levels was carried out as previouslydescribed (Audhya et al., 2000; Rudge et al., 2004). Briefly,cells were grown in synthetic medium with the appropriate aminoacids. Cells from an early log phase culture were harvested,washed, and resuspended in inositol-free synthetic medium (IFM).Cells were shifted to the appropriate temperature (26 or 38°C)for 10 min and labeled with 60 µCi of myo-[2-³H]inositol(Amersham Biosciences, Piscataway, NJ) in IFM for an additional45 min. Phosphoinositides were extracted by ice-cold precipitationwith a final concentration of 4.5% perchloric acid and deacylatedby treatment with methylamine. Extracts of deacylated lipidswere further processed as described in Rudge et al. (2004).[³H]glycerol-phosphoinositides were separated using an anion-exchangePartisphere SAX column (Whatman, Clifton, NJ) coupled to a GOLDHPLC system (Beckman Coulter, Fullerton, CA) and quantitatedby liquid scintillation counting using an on-line radiomaticdetector (Packard Instrument Co., Meriden, CT) utilizing UltimaFlo scintillation fluid (Packard).

Metabolic Labeling and Immunoprecipitation
Cell labeling and immunoprecipitations were performed as previouslydescribed (Audhya et al., 2000). Log-phase cultures were concentratedto 5 OD600/ml and labeled with 2 µl/OD600 Trans-³⁵S labelmix (DuPont New England Nuclear, Boston, MA) for 10 min in YNB,supplemented with 2% glucose, appropriate amino acids, and 100µg/ml bovine serum albumin. Cells were chased with anexcess of unlabeled methionine/cysteine for the indicated times,and proteins were precipitated with 9% trichloroacetic acid(TCA) on ice. For temperature shift experiments, cells wereshifted to the appropriate temperature for 10–30 min beforelabeling. For analysis of media-secreted proteins, cells wereseparated from media by gentle centrifugation before precipitation.Extracts were immunoprecipitated with antisera against CPY (Cowleset al., 1997) or Gas1p (R. Schekman, UC Berkeley). Immunoprecipitatedproteins were resuspended in sample buffer, resolved by SDS-PAGE,and subjected to autofluorography.

Miscellaneous
Western blot analysis of SDS-PAGE–resolved proteins wereperformed as previously described (Rudge et al., 2004). GFPand HA fusion proteins were detected using mouse monoclonalantibodies against GFP (Santa Cruz Biotechnology, Santa Cruz,CA) and HA (12CA5; Roche). Antibody against G6PDH was purchasedfrom Sigma (St. Louis, MO). Immunoreactive proteins were detectedusing horseradish peroxidase–conjugated goat anti-mouseor anti-rabbit (Zymed Laboratories, South San Francisco, CA)and SuperSignal chemiluminescent substrate (Pierce Chemical,Rockford, IL).

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

SGA Analysis Reveals a Network of PIK1 Genetic Interactions
To identify components of the Pik1p-dependent secretory apparatusrequired during transport out of the Golgi, we conducted a syntheticgenetic interaction screen (Tong et al., 2001) using a yeaststrain expressing a functionally impaired temperature-sensitiveallele of pik1. From such a sensitized genetic screen, we anticipatedthat we would identify gene products essential for Pik1p-dependentpathways. We used error-prone PCR mutagenesis targeted to thecatalytic kinase domain of Pik1p, to engineer the pik1-139^tsmutant strain that could grow robustly up to temperatures of35°C. Under permissive conditions (26°C), pik1-139^tscells have a modest 20% reduction in PtdIns(4)P levels (SEY6210;0.88 ± 0.06% compared with pik1-139^ts; 0.70 ±0.06% of PtdIns labeled). Accordingly, at 26°C, pik1-139^tscells lack any detectable growth defects associated with theloss of PtdIns(4)P signaling. Previously, it was shown thatPik1p and Stt4p each contribute $~$ 50% of the total cellular PtdIns(4)P(Audhya et al., 2000). As such, at the nonpermissive temperature(38°C, see Audhya et al., 2000), pik1-139^ts cells have 43%reduced levels of PtdIns(4)P (SEY6210; 0.99 ± 0.08% comparedwith pik1-139^ts; 0.56 ± 0.08% of PtdIns labeled) andconsequentially accumulate exaggerated Golgi as well as othermembranous structures (unpublished data). Most of the remainingPtdIns(4)P observed in pik1-139^ts cells grown under nonpermissiveconditions is due to the unaltered PtdIns 4-kinase activityof Stt4p (Audhya et al., 2000 and unpublished data). These resultsare consistent with the proposed role for Pik1p-generated PtdIns(4)Pin Golgi structure/function (Hama et al., 1999; Walch-Solimenaand Novick, 1999; Audhya et al., 2000).

The pik1-139^ts strain was then individually crossed with $~$ 4700single deletion strains that represent the complete set of viablehaploid deletion mutants in S. cerevisiae. Double mutants exhibitingreduced growth at 26°C relative to the parental strainswere scored three independent times. The results of the screenare listed in Supplementary Table 1. More than 30 genes, whendeleted in the pik1-139^ts background, displayed a syntheticgrowth defect. The pik1 interactions were highly enriched forgenes with roles in membrane trafficking (Supplementary Table1 and Figure 1A), indicative of an essential function for Pik1pin secretion. Consistent with previous studies suggesting rolesfor Pik1p/PtdIns(4)P in cytokinesis (Garcia-Bustos et al., 1994),actin rearrangement (Walch-Solimena and Novick, 1999) and vacuolefunction (Audhya et al., 2000), several genes involved in theseprocesses were isolated. Surprisingly, gene products with knownPtdIns(4)P-binding modules, such as a pleckstrin homology (PH)domain (Yu et al., 2004), were not isolated. Further analysisof results obtained from this study and published studies revealedmultiple interactions within subsets of genes involved in anterogradeand retrograde Golgi traffic (Figure 1A).

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Figure 1. Phosphoinositide kinase specific genetic interactions. (A) Schematic of genes identified by SGA involved in membrane trafficking with known genetic interactions (synthetic sick or lethal). (B) Genetic interactions of four trafficking genes obtained from SGA (drs2 ${Delta}$ , ypt31 ${Delta}$ , kre11 ${Delta}$ , and trs33 ${Delta}$ ) were analyzed in pik1-139^ts, pik1–83^ts, stt4^ts, and mss4^ts. Tetrads were isolated at 26°C and the growth of the double mutants was assessed at 26°C. +/-; reduced growth, ++; similar to growth of single mutants. Temperature at which lethality is observed is given in parentheses.

Specific Interactions with the Pik1p PtdIns 4-kinase
SGA analysis identified four genes: DRS2, TRS33, KRE11, andYPT31, with previous ascribed roles in Golgi anterograde traffickingto the plasma membrane. Drs2p, a Golgi-associated, integralmembrane aminophospholipid translocase, is required for generatingclathrin-coated exocytic vesicles (Chen et al., 1999; Gall etal., 2002). TRS33 and KRE11 encode nonessential subunits ofthe TRAPPII, a large Golgi-associated complex consisting of10 proteins (Bet3p, Bet5p, Trs20p, Trs23p, Trs31p, Trs33p, Trs85p,Kre11p, Trs120p, and Trs130p; Sacher et al., 2001). Temperature-sensitivemutants of the essential subunits display severe secretion defects,as well as an accumulation of aberrant Golgi structures (Sacheret al., 2001). YPT31 encodes a member of the Ypt/rab familyof GTPases that is required for secretory transport, possiblyby regulating vesicle formation at the trans-Golgi (Benli etal., 1996; Jedd et al., 1997).

Deletion of DRS2, TRS33, KRE11, or YPT31 in either the pik1-139^tsor another temperature-sensitive allele of PIK1, pik1–83^tsstrain (Hama et al., 1999; Audhya et al., 2000) resulted ineither lethality or a severe growth defect (Figure 1B). AlthoughYpt31p shares 81% sequence identity with Ypt32p, only YPT31was uncovered in our SGA analysis using the pik1^ts mutation.Consistent with this observation, pik1-139^ts ypt32 ${Delta}$ double mutantcells did not exhibit a significant synthetic growth defect(lethality at 34°C) in contrast to pik1-139^ts ypt31 ${Delta}$ doublemutant cells (Figure 1B). Because Ypt31p is more abundant thanYpt32p in the cell (Jedd et al., 1997), these data suggest thatYpt31p may play a more dominant role in cells compared withYpt32p.

We next compared the specificity of the genetic interactionsobtained by SGA analysis by examining the effects of deletingthese genes in strains harboring temperature-sensitive Stt4p,the second essential PtdIns 4-kinase in yeast, and Mss4p, theessential yeast PtdIns(4)P 5-kinase. As shown in Figure 1B,no significant genetic interactions with these PtdIns-kinaseswere identified. The PtdIns-kinase specificity of these geneticinteractions suggests roles for Drs2p, Trs33p, Kre11p, and Ypt31pin a common or parallel pathway to Pik1p in Golgi function.

Coordinated Regulation of the Secretory Pathway by Pik1p and Ypt31p
It has become increasingly apparent that cooperative protein-phosphoinositideand protein-protein interactions are required for the localizationof specific signaling molecules to their site of action (Levineand Munro, 2002). For instance, localization of early endosomeantigen 1 to the endosome requires its interaction with bothactive, GTP-bound Rab5 (Simonsen et al., 1998), and PtdIns(3)P(Burd and Emr, 1998). In accordance with this model, we hypothesizedthat active, GTP-bound Ypt31p, and Pik1p-generated PtdIns(4)Pmay recruit effector molecules to function at the Golgi. Wefirst investigated the phenotypes of pik1-139^ts ypt31 ${Delta}$ doublemutant cells to determine whether specific membrane traffickingpathways were attenuated in these cells. Growth and organellemorphology of pik1-139^ts cells (grown at the permissive temperature)or ypt31 ${Delta}$ cells (Benli et al., 1996; Jedd et al., 1997) weresimilar to wild-type cells. However, electron microscopy ofpik1-139^tsypt31 ${Delta}$ double mutant cells grown under the same conditions(26°C) revealed an accumulation of abnormal Golgi structures,including Berkeley bodies, and fragmented vacuoles (unpublisheddata), indicating a synthetic defect in Golgi function.

We next investigated the localization of proteins that trafficfrom the Golgi to the plasma membrane. Snc1p is a yeast SNAREthat mediates the fusion of exocytic vesicles with the plasmamembrane (Protopopov et al., 1993). Snc1p, which localizes tothe plasma membrane at sites of bud formation, undergoes rapidendocytosis into early endocytic structures and is recycledto the Golgi where it is incorporated into another round ofsecretory vesicles (Lewis et al., 2000). Consistent with previousstudies (Lewis et al., 2000), wild-type cells expressed GFP-Snc1pat the plasma membrane of newly formed daughter cells, and atthe mother-daughter neck (Figure 2A). A few punctate structureswere also visible, consistent with the dynamic recycling ofthis SNARE to and from the Golgi complex. Similar localizationpatterns of GFP-Snc1p fluorescence were also seen in ypt31 ${Delta}$ andpik1-139^ts cells at the permissive temperature (Figure 2A).In pik1-139^tsypt31 ${Delta}$ double mutant cells grown at the permissivetemperature (26°C), the polarized plasma membrane localizationof GFP-Snc1p was no longer observed, and instead GFP-Snc1p residedin punctate structures, some of which resembled "swollen Golgi,"whereas others resembled tubular rings (Figure 2A). These datasuggest that Pik1p and Ypt31p are required for GFP-Snc1p recyclingto and/or secretion from the Golgi.

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Figure 2. Trafficking of Snc1p and Chs3p requires Pik1p and Ypt31p. (A) GFP-Snc1p or (B) Chs3p-GFP distribution at 26°C in live cells, either wild-type (Wt) or carrying the indicated mutation, ypt31 ${Delta}$ , pik1-139^ts, and pik1-139^ts ypt31 ${Delta}$ . Arrows indicate bud necks and arrowheads indicate bud tips. (B) Chs3p-GFP transport to the cell surface was monitored by blocking endocytosis with LatA (200 µM, Molecular Probes) or treated with vehicle (dimethyl sulfoxide) as described in Valdivia et al. (2002

Chitin synthase III (Chs3p), a cell surface enzyme necessaryfor cell wall assembly, follows a recycling pattern similarto that of Snc1p. Chs3p localizes to the cell surface, to themother-bud junction, and to intracellular punctate structures,referred to as chitosomes (Valdivia et al., 2002). Because chitosomesresemble early endosomes and Chs3p follows a trafficking pathwaysimilar to Snc1p (Lewis et al., 2000; Valdivia et al., 2002),we next determined whether the transport of Chs3p to the budneck required Pik1p and/or Ypt31p. Chs3p tagged with GFP atits C-terminus was previously found to be fully functional (Schorret al., 2001; Valdivia et al., 2002). We examined the localizationof Chs3p, chromosomally tagged with GFP (Figure 2B). In 48%of budded wild-type cells, Chs3p-GFP localized to the mother-budneck. A modest decrease in the targeting of Chs3p-GFP to thebud neck was observed in ypt31 ${Delta}$ cells (39% of budded cells).Chs3p-GFP was localized to the bud neck in only 22% of buddedpik1-139^ts cells at the permissive temperature (26°C), suggestingthat Pik1p/PtdIns(4)P is required for proper Chs3p targeting.Consistent with the defect in GFP-Snc1p localization (Figure 2A),<1% of budded pik1-139^ts ypt31 ${Delta}$ double mutant cells (26°C)expressed Chs3p-GFP at the bud neck; Chs3p mostly accumulatedintracellularly (Figure 2B). We also monitored the transportof Chs3p-GFP to the plasma membrane by blocking endocytosiswith LatA (Figure 2B). Consistent with a defect in Golgi toplasma membrane traffic, Chs3p-GFP remained predominately inintracellular structures in pik1-139^ts ypt31 ${Delta}$ double mutant cellstreated with LatA (Figure 2B). These results provide evidencefor a functional interaction between Pik1p and Ypt31p in Golgito plasma membrane traffic.

We next examined the localization of other plasma membrane proteinsthat unlike Snc1p and Chs3p are trafficked to and degraded inthe vacuole in response to environmental conditions. Consistentwith previous reports (Malinska et al., 2003), the plasma membranehexose transporter, Hxt1p, localized uniformly at the plasmamembrane, with some fluorescence localized to punctate structuresand/or the vacuole in wild-type cells (Figure 3A). This patternof Hxt1p-GFP localization was also observed in ypt31 ${Delta}$ cells,pik1-139^ts cells, and pik1-139^tsypt31 ${Delta}$ double mutant cells, demonstratingthat transport of Hxt1p from the Golgi to the plasma membranewas unaffected (Figure 3A). We also examined the localizationof another plasma membrane transporter, the tryptophan permease,Tat2p, chromosomally tagged with GFP to circumvent potentialtrafficking artifacts due to overexpression. Tat2p-GFP, likeHxt1p-GFP, is expressed uniformly at the plasma membrane withpunctate and/or vacuole fluorescence observed in some cells(Umebayashi and Nakano, 2003 and Figure 3A). Under permissivegrowth conditions, the localization of Tat2p-GFP in ypt31 ${Delta}$ cells,pik1-139^ts cells, and pik1-139^tsypt31 ${Delta}$ double mutant cells didnot change relative to wild-type cells (Figure 3A). Additionally,the processing of several cargo proteins, the soluble vacuolarcarboxypeptidase Y (CPY), and a glycophospholipid-anchored surfaceprotein (Gas1p) were unaffected in ypt31 ${Delta}$ cells, pik1-139^ts cells,and pik1-139^tsypt31 ${Delta}$ double mutant cells relative to wild-typecells (Figure 3B). Collectively, these results provide evidencefor a functional interaction between Pik1p and Ypt31p in thespecific targeting of proteins that continuously recycle duringpolarized growth.

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Figure 3. Trafficking competence of pik1-139^ts ypt31 ${Delta}$ double mutant cells at permissive temperature. (A) Hxt1p-GFP and Tat2p-GFP distribution at 26°C in Wt, ypt31 ${Delta}$ , pik1-139^ts, and pik1-139^ts ypt31 ${Delta}$ . (B) Indicated yeast strains (Wt, ypt31 ${Delta}$ , pik1-139^ts, and pik1-139^ts ypt31 ${Delta}$ ) were metabolically labeled with Tran-³⁵S for 10 min, and chased in the presence of excess methionine/cysteine for 30 min at 26°C. CPY and Gas1p were immunoprecipitated from cell lysates, resolved by SDS-PAGE, and visualized by fluorography. p, precursor form; m, mature form.

Pik1p and Ypt31p Function in a Common Set of Trafficking Pathways
If Pik1p and Ypt31p function in similar trafficking pathways,then inactivation of Ypt31p should display similar defects inmembrane traffic as the inactivation of Pik1p. To test our hypothesis,we generated a temperature-sensitive mutant of Ypt31p and thencompared the phenotypes with those seen during the inactivationof Pik1p, in the same strain background, SEY6210. As previouslymentioned, Ypt31p shares a high degree of sequence similaritywith the Ypt32p GTPase, and deletion of both genes is lethal,indicating functional redundancy (Benli et al., 1996; Jedd etal., 1997). We therefore generated new temperature-sensitivealleles of YPT31 by first mutating the ORF by random PCR mutagenesisand then integrating, via homologous recombination, the mutatedPCR products into the genome of ypt32 ${Delta}$ mutant cells. We isolatedtwo strains that exhibited temperature-sensitive growth. Thestrain, ypt32 ${Delta}$ ypt31-101^ts that grew most robustly at 26°Cwas characterized further. ypt32 ${Delta}$ ypt31-101^ts double mutant cellsare temperature-sensitive for growth at elevated temperatures(>37°C), which can be fully rescued by the introductionof wild-type YPT31 expressed from a low-copy plasmid (Figure 4A).

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Figure 4. Pik1p and Ypt31p act in similar biological pathways. (A) Temperature-sensitive growth of yeast expressing ypt31-101^ts in ypt32 ${Delta}$ background is rescued by expressing low-copy YPT31. (B and C) Wt, ypt32 ${Delta}$ , and ypt32 ${Delta}$ ypt31-101^ts double mutant cells were incubated at the indicated temperature for 10 or 30 min, metabolically labeled with Tran-³⁵S for 10 min, and chased in the presence of excess methionine/cysteine for 30 min. CPY and Gas1p were analyzed as described in the legend to Figure 3. To assay for general secretion competence, cells and media were separated by centrifugation, and proteins secreted into the media during the pulse-chase were visualized by SDS-PAGE and fluorography. (D) ypt32 ${Delta}$ ypt31-101^ts double mutant cells expressing GFP-Snc1p were grown to early/midlog phase, shifted to 26°C or 38°C for 30 min, and observed by fluorescence microscopy.

To further characterize ypt32 ${Delta}$ ypt31-101^ts double mutant cells,we assessed the anterograde secretory transport of CPY and Gas1p.At the permissive temperature, CPY transport to the vacuolewas unaffected (Figure 4B). However, after a 10- or 30-min shiftto the restrictive temperature (38°C), CPY was predominatelyin the Golgi-modified form (p2) with minor amounts in the ER-modified(p1) and mature (m) forms. Gas1p acquires a glycophosphoinositollinkage in the ER (p) and is then glycosylated in the Golgi(m) before its transport to the plasma membrane. Although amodest defect is observed at the permissive temperature, shiftingof ypt32 ${Delta}$ ypt31-101^ts double mutant cells to the nonpermissivetemperature (38°C, for 10 or 30 min) resulted in the accumulationof the ER-modified form (p) of Gas1p (Figure 4B). Expressionof YPT31 in the ypt32 ${Delta}$ ypt31-101^ts double mutant cells resultedin full suppression of CPY and Gas1p trafficking defects (Figure 4B).We also examined general secretion competence of ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells, by taking advantage of the fact that onlya few yeast proteins are efficiently secreted into the growthmedium (Robinson et al., 1988). As expected, at the nonpermissivetemperature, ypt32 ${Delta}$ ypt31-101^ts double mutant cells exhibiteda near complete block in protein secretion into the medium,whereas double mutant cells expressing wild-type Ypt31p exhibiteda normal pattern of protein secretion (Figure 4C). ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells at the nonpermissive temperature (38°Cfor 30 min) also accumulated GFP-Snc1p intracellularly, whereasypt32 ${Delta}$ ypt31-101^ts double mutant cells at the permissive temperaturehad only a partial defect in the polarized membrane localizationof GFP-Snc1p (Figure 4D). These results reinforce the requirementof a functional Golgi for efficient Snc1p recycling. Collectively,the Golgi transport phenotypes observed upon Ypt31/32p inactivationresemble those observed when Pik1p is inactivated (Audhya etal., 2000), suggesting that these proteins are involved in similarbiological functions at the Golgi, consistent with the geneticinteractions identified by our SGA analysis.

Ypt31/32 Does Not Regulate PtdIns(4)P Synthesis or Pik1p Localization
Because our genetic and phenotypic analysis suggests that Ypt31pand Pik1p functionally interact in specific biological pathways,it is possible that Ypt31p acts upstream of Pik1p by stimulatingthe kinase activity of Pik1p and/or by recruiting Pik1p to theGolgi. We next determined the levels of PtdIns(4)P under conditionswhere Ypt31/32p is transiently inactivated. ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells were grown at the permissive temperature(26°C) and then shifted to the nonpermissive temperature(38°C) for 10 min before labeling with myo-[³H]inositolfor an additional 45 min at 38°C. Subsequent analysis of[³H]inositol–labeled lipids revealed no significant changesin the amounts of PtdIns(4)P at the nonpermissive temperature(Figure 5). This result suggests that the inactivation of Ypt31/32pdoes not alter production of PtdIns(4)P and therefore does notappear to regulate PtdIns 4-kinase activity in cells. Additionally,overexpression of YPT31 or a GTPase-deficient mutant, ypt31Q72L, does not restore the temperature-sensitive growth defectof pik1^ts cells, nor does it affect PtdIns(4)P levels in wild-typeor ypt31 ${Delta}$ cells (unpublished data). A 4.5-fold increase in PtdIns(3,5)P₂was observed (SEY6210; 0.12 ± 0.02%; ypt32 ${Delta}$ ; 0.16 ±0.03%; ypt32 ${Delta}$ ypt31-101^ts; 0.54 ± 0.11% of PtdIns labeled),and concurrently the vacuoles in ypt32 ${Delta}$ ypt31-101^ts double mutantcells are highly fragmented (unpublished data), consistent withthe role for PtdIns(3,5)P₂ in vacuolar membrane morphology (Rudgeet al., 2004). The levels of PtdIns(4,5)P₂ are significantlyreduced by 2.8-fold (SEY6210; 2.13 ± 0.18%; ypt32 ${Delta}$ ; 2.39± 0.04%; ypt32 ${Delta}$ ypt31-101^ts; 0.77 ± 0.18% of PtdInslabeled) at the nonpermissive temperature (38°C). The underlyingbasis of the elevated PtdIns(3,5)P₂ levels and the reduced PtdIns(4,5)P₂levels is not clear. One possibility is that the observed accumulationof Golgi membranes and inappropriate sorting of several proteinsmay indirectly affect the distribution of the kinases and phosphatasesinvolved in maintaining the levels of PtdIns(3,5)P₂ and PtdIns(4,5)P₂in ypt32 ${Delta}$ ypt31-101^ts double mutant cells.

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Figure 5. Phosphoinositide levels in Wt, ypt32 ${Delta}$ , and ypt32 ${Delta}$ ypt31-101^ts double mutant cells. Cells were incubated at the temperature indicated for 10 min and labeled with myo-[2-³H]inositol for 45 min, and phosphoinositides were analyzed as previously described in Rudge et al. (2004

). The levels of each indicated phosphoinositide are expressed as a percentage of the total ³H-labeled phosphoinositides analyzed by HPLC and represent the average of two independent experiments done in duplicate (n = 4).

We next epitope-tagged Pik1p with GFP to observe the cellularlocalization of GFP-Pik1p under conditions where Ypt31p is transientlyinactivated. Haploid pik1 ${Delta}$ cells expressing GFP-Pik1p from alow-copy plasmid (as the only source of PIK1) were generated,indicating that GFP-Pik1p is functional. In wild-type backgrounds,GFP-Pik1p fluorescence localizes predominantly to concentratedpuncta that colocalized with a Golgi marker protein, Sec7p (Figure 6A).Our observed localization of GFP-Pik1p is consistent withthe primary role of Pik1p in Golgi structure and function. Inypt32 ${Delta}$ ypt31-101^ts mutant background at both the permissive andnonpermissive temperatures, GFP-Pik1p remained associated withpunctate structures (Figure 6A), demonstrating that a functionalYpt31/32p is not required for Pik1p to associate with intracellularmembranes. Because overexpression of Sec7p in ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells has adverse effects on growth (Jones etal., 1999), we were unable to determine whether the fluorescentpuncta of GFP-Pik1p and Sec7p-DsRED colocalized. These datasuggest that Ypt31p does not function as an upstream regulatorof Pik1p kinase activity or localization.

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Figure 6. Independent localization of Pik1p and Ypt31p to the trans-Golgi network. (A) pik1 ${Delta}$ cells expressing GFP-Pik1p and Sec7p-DsRed were examined by fluorescence microscopy at 26°C. ypt32 ${Delta}$ ypt31-101^tspik1 ${Delta}$ cells expressing GFP-Pik1p were grown at 26°C or shifted for 1 h at 38°C and examined by fluorescence microscopy. (B) ypt31 ${Delta}$ ypt32 ${Delta}$ cells expressing GFP-Ypt31p and Sec7p-DsRed were grown at 26°C and examined by fluorescence microscopy. (C) Wild-type (PIK1), pik1–83^ts, or pik1-139^ts (unpublished data) cells expressing GFP-YPT31 from a low copy plasmid and Sec7p-DsRed were grown at 26°C (unpublished data) or shifted 1 h at 38°C and examined by fluorescence microscopy.

Ypt31p Colocalizes with Sec7p at the trans-Golgi
Ypt31/32p has been reported to have a punctate distributionlike that of the Golgi (Benli et al., 1996; Jedd et al., 1997),and we confirmed this using a functional GFP-tagged versionof Ypt31p (Figure 6B). Furthermore, we extended this observationby demonstrating that GFP-Ypt31p localization was concentratedto Sec7p-containing compartments, indicative of trans-Golgilocalization (Figure 6B). Similar to a previous report (Jeddet al., 1997), GFP-Ypt31p fluorescence appeared to have a polarizeddistribution, being concentrated at the emerging bud or smallbud tip in rapidly dividing cells (unpublished data). This localizationpattern of Ypt31p is most consistent with the observations thatlate Golgi can preferentially localize to sites of polarizedgrowth (Rossanese et al., 2001).

We next investigated whether the localization of GFP-Ypt31pto the Golgi is mediated by Pik1p-generated PtdIns(4)P. WhenGFP-Ypt31p is expressed in yeast with a temperature-sensitiveallele of pik1, incubation of cells at a nonpermissive temperature,which causes a substantial reduction in PtdIns(4)P (Audhya etal., 2000 and this study) did not affect the localization ofGFP-Ypt31p at Sec7p-enriched puncta compared with that of wild-typePIK1 control cells (Figure 6C). These data indicate that Ypt31pdoes not require Pik1p kinase activity for normal membrane recruitment.We did note that the mobility of Sec7p/Ypt31p-positive compartmentswas reduced in pik1–83^ts cells when shifted to the nonpermissivetemperature, and as a result of the reduced membrane dynamics,we were able to observe significant colocalization of GFP-Ypt31pfluorescence to Sec7p-labeled Golgi (Figure 6B). Taken together,the above results are consistent with a coordinated functionof Ypt31p and Pik1p at a common membrane compartment, the trans-Golgi.

TRAPPII Functions Upstream of Ypt31
Previous studies have demonstrated that overexpression of YPT31can suppress the lethality of trs130, which encodes an essentialTRAPPII component (Yamamoto and Jigami, 2002; Zhang et al.,2002), suggesting a functional relationship between TRAPPIIand Ypt31p. TRS33 and KRE11 are nonessential subunits of theTRAPPII complex and were identified in our SGA analysis as havinga functional interaction with pik1. To provide additional evidencethat TRAPPII functions in Ypt31p signaling, we took advantageof our observation that deletion of KRE11 in trs33 ${Delta}$ cells waslethal and tested whether the lethality of kre11 ${Delta}$ trs33 ${Delta}$ doublemutants could be suppressed by the overproduction of YPT31.Haploid trs33 ${Delta}$ and kre11 ${Delta}$ single deletion mutants of oppositemating types, each expressing YPT31 were mated and sporulatedand tetrads were isolated. As shown in Figure 7A, kre11 ${Delta}$ trs33 ${Delta}$ double mutants were never isolated. We next made a point mutationin YPT31 to mimic the active, GTP-bound state (Walworth et al.,1989) and expressed this mutant, ypt31 Q72L, in both haploidtrs33 ${Delta}$ and kre11 ${Delta}$ single deletion mutants. Surprisingly, kre11 ${Delta}$ trs33 ${Delta}$ double mutants were now isolated only when ypt31 Q72Lwas overexpressed (Figure 7A). Consistent with previous findings(Zhang et al., 2002), overexpression of YPT31 in a trs130 ${Delta}$ (andto a lesser extent trs120 ${Delta}$ ) deletion strains rescued the lethalityin the SEY6210 background (Figure 7A). However, we found thattrs120 ${Delta}$ deletion mutants obtained from trs120 ${Delta}$ heterozygotes grewbetter when YPT31 was overexpressed in its GTP-locked form.Our data demonstrate that activated Ypt31p suppresses the mutantgrowth phenotypes exhibited by trs130 ${Delta}$ mutants, trs120 ${Delta}$ mutants,and kre11 ${Delta}$ trs33 ${Delta}$ double mutants.

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Figure 7. GTP-dependent suppression of TRAPPII lethality and trafficking defects by YPT31. (A) Tetrad analysis of diploid strains were transformed with high-copy wild-type YPT31, or ypt31 Q72L, sporulated, and dissected on YPD plates at 26°C. Haploid cells with deleted gene(s) carrying either YPT31 or ypt31 Q72L are circled (confirmed by PCR and growth on selection media). (B) trs130-HA^ts (33 aa deleted from C-terminus of TRS130, and tagged with HA) was examined for temperature-sensitive growth when expressing low (cen) or high (2 µ) copies of YPT31 or ypt31 Q72L. (C) Wt, TRS130-HA, or trs130-HA^ts cells expressing vector, YPT31 or ypt31 Q72L, were incubated at 26 or 38°C for 30 min, metabolically labeled with Tran-³⁵S for 10 min, and chased in the presence of excess methionine/cysteine for 30 min. CPY and GAS1p were analyzed as described in the legend to Figure 3. (D) General secretion competence was analyzed as described in the legend to Figure 4.

To characterize the genetic interaction of YPT31 and TRS130further, we constructed a temperature-sensitive mutant of TRS130by deleting the 33 amino acids from the C terminus as describedby Sacher et al. (2001). Temperature-sensitive growth of trs130-HA^tsmutant cells could be suppressed when cells expressed eitherwild-type or GTP-locked forms of YPT31, similar to the suppressionobserved in the trs130 ${Delta}$ deletion mutants (Figure 7B). We nextexamined whether the expression of YPT31 could suppress thetrafficking defects associated with inactivation of TRAPPII.In trs130-HA^ts mutant cells shifted to the restrictive temperature,the majority of CPY was detected as a mixture of p1, p2, andmature forms, indicative of a defect in CPY trafficking outof the Golgi. Similarly, trs130-HA^ts mutant cells exhibiteda defect in the processing of Gas1p at the nonpermissive temperature.Expression of YPT31 from a low-copy plasmid, which partiallysuppressed the growth phenotype (Figure 7B), resulted in partialsuppression of the CPY and Gas1p trafficking defect (Figure 7C).However, expression of ypt31 Q72L from a low-copy plasmid,which suppresses the growth phenotype (Figure 7B), resultedin near complete suppression of the CPY and Gas1p traffickingdefect (Figure 7C). Lastly, trs130-HA^ts mutant cells at thenonpermissive temperature exhibit a strong block in proteinsecretion, whereas trs130-HA^ts mutant cells expressing wild-typeYPT31 or ypt31 Q72L secreted proteins into the medium, similarto that of wild-type cells (Figure 7D). Moreover, expressionof a nucleotide-free mutant of YPT31, ypt31 N126I was lethalwhen expressed in trs130-HA^ts mutant cells (unpublished data).Collectively, these results support a role for TRAPPII functioningupstream of Ypt31p, potentially participating in the activationof Ypt31p.

Gyp2p Functions as a GAP for Ypt31p In Vivo
To provide additional evidence that TRAPPII functions upstreamof Ypt31p, we reasoned that deletion of a specific rab-GAP wouldprolong the activated state of Ypt31p and thereby shift endogenousYpt31p to an activated, GTP-bound state, analogous to the expressionof ypt31 Q72L, which mimics the active, GTP-bound state (Figure 7).To date, a GAP for Ypt31p has not been identified. However,a similar approach was successful in identifying Gyp1p, a cis-Golgilocalized protein, as the GAP for Ypt1p (Du and Novick, 2001),a rab-GTPase functioning in ER to Golgi transport. Deletionof either GYP1 or a related homologue, GYP2, in wild-type cellsdid not have any effect on growth or trafficking (Figure 8Aand unpublished data). Deletion of the GYP1 in the trs130-HA^tsmutant cells failed to suppress the growth defect at the nonpermissivetemperature (Figure 8A), suggesting that Gyp1p does not exertsignificant GAP activity toward Ypt31p, which is consistentwith in vitro studies (Albert et al., 1999). It has been documentedthat Gyp2p has relatively low GAP activity toward Ypt31p invitro (Albert and Gallwitz, 1999). Surprisingly, deletion ofGYP2 in trs130-HA^ts mutant cells restored growth at the nonpermissivetemperature of 37°C (Figure 8A) and partially at 38°C(unpublished data). Consistent with the restoration of growthat 37°C, deletion of GYP2 also suppressed the traffickingdefects (CPY, Gas1p, and HSP150 secretion) associated with theloss of Trs130p function (unpublished data).

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Figure 8. Gyp2p is a GAP for Ypt31p in vivo. (A) gyp2 deletion suppresses the temperature-sensitive growth of trs130-HA^ts. (B) SEC4 and YPT6 (high-copy) do not suppress the temperature-sensitive growth defect of trs130-HA^ts. (C) gyp2 deletion suppresses the temperature-sensitive growth of ypt32 ${Delta}$ ypt31-101^ts double mutant cells. (D) gyp2 deletion specifically rescues trafficking defects of ypt32 ${Delta}$ ypt31-101^ts double mutant cells. ypt32 ${Delta}$ ypt31-101^ts, ypt32 ${Delta}$ ypt31-101^ts gyp1 ${Delta}$ , and ypt32 ${Delta}$ ypt31-101^tsgyp2 ${Delta}$ were incubated at 37°C for 30 min, metabolically labeled with Tran-³⁵S for 10 min, and chased in the presence of excess methionine/cysteine for the indicated minutes. CPY and Gas1p were analyzed as described in the legend to Figure 3.

It has been previously demonstrated that Gyp2p has high in vitroGAP activity toward Sec4p (which regulates the traffic and fusionof post-Golgi vesicles to the plasma membrane; Salminen andNovick, 1987) and Ypt6p (which regulates the fusion of lateendocytic vesicles to the trans-Golgi; Siniossoglou and Pelham,2001). Therefore, in order to eliminate the possibility thatthe suppression observed in gyp2 ${Delta}$ trs130-HA^ts double mutant cellsis due to the activity of Gyp2p toward Sec4p and/or Ypt6p, wedetermined whether the overexpression of either SEC4 or YPT6could suppress the temperature-sensitive growth of trs130-HA^tsmutant cells. However, no suppression of the trs130-HA^ts mutantcells was observed when the wild-type or GTPase-deficient formsof SEC4 or YPT6 were expressed (Figure 8B and unpublished data).Our results suggest that Gyp2p functions as a physiologicallyrelevant GAP for Ypt31p and that GAP activities measured invitro may not reveal a true in vivo rab target.

Having demonstrated a role for Gyp2p as a potential GAP forYpt31p in vivo, we rationalized that deletion of GYP2 mightalso suppress the growth and trafficking defects of ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells. As anticipated, deletion of GYP2, but notGYP1, suppressed the growth defect of ypt32 ${Delta}$ ypt31-101^ts doublemutant cells fully at 37°C (Figure 8C) and partially at38°C (unpublished data). More significantly, deletion ofGYP2 and not GYP1, suppressed the defects of CPY and Gas1p processingin ypt32 ${Delta}$ ypt31-101^ts double mutant cells grown at 37°C (Figure 8D).This result demonstrates that the deletion of GYP2 canalleviate the trafficking defects associated with loss of Ypt31p-dependentGolgi function.

GYP2, Conserved Member of GRAM-Domain Family of rab-GAPs
Most of the known rab GAPs share a region of homology, referredto as the TBC (Tre2, Bub2, Cdc16) domain (Neuwald, 1997), encodingthe core catalytic machinery for GTPase activity (Albert etal., 1999). The S. cerevisiae genome contains 11 genes encodingTBC/rab-GAP domain proteins. Compared with the other rab-GAPdomain-containing proteins in yeast, Gyp2p is the only rab-GAPrecognized to contain any additional protein motifs. In additionto a TBC/rab-GAP domain, protein motif search using SMART (Schultzet al., 2000) revealed a GRAM (Glucosyltransferases, Rab-likeGTPase activators, and Myotubularian) domain and an EfHand withinGyp2p (Figure 9A). Additional database searches revealed thatthe domain organization of Gyp2p is evolutionarily conserved,with putative orthologues in human (VRP and KIAA0676), Drosophila(CG7324) and Caenorhabditis elegans (Y45F10A.6; Figure 9A).This suggests that Gyp2p may represent a member of a uniqueset of conserved rab-GAPs.

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Figure 9. Gyp2p requires its GRAM domain and GAP activity for function in cells. (A) Schematic representation of the conserved domains in Gyp2 family in human, Drosophila, C. elegans, and yeast. EfH, EfHand; cc, coiled-coil. (B) Serial dilution of yeast cells expressing wild-type or mutants of GYP2 from low-copy plasmids at 26 and 37°C. (C) trs130-HA^ts gyp2 ${Delta}$ cells expressing GFP-GYP2, GFP-gyp2 G80E, or GFP-gyp2 R295K from low-copy plasmids were grown at 26°C and shifted to 37°C for 1 h, and total cellular protein content were TCA-precipitated and resolved by Western blotting. Glucose 6-phosphate dehydrogenase (G6PDH) was examined as a loading control.

To determine the in vivo functionality of the domains in Gyp2p,we developed an assay system based on our observation that deletionof GYP2 restored the growth of the trs130-HA^ts and ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells at 37°C (Figure 8). Suppression of thetemperature-sensitive growth of the trs130-HA^ts and ypt32 ${Delta}$ ypt31-101^tsdouble mutant cells conferred by deleting GYP2 is abrogatedby the expression of wild-type GYP2 from a low-copy plasmid(Figure 9B), demonstrating that GYP2 expresses a functionalprotein and reinforces Gyp2p as a negative regulator of Ypt31p.To confirm that the GAP activity of Gyp2p is required for itsin vivo function, we mutated the invariable arginine residuein the catalytic TBC/rabGAP domain (R295) that is predictedto be essential for GAP activity (Albert et al., 1999). Expressionof gyp2 R295K from a low copy plasmid in the gyp2 ${Delta}$ trs130-HA^tsor gyp2 ${Delta}$ ypt32 ${Delta}$ ypt31-101^ts mutant cells, failed to restore Gyp2pGAP function as shown by the ability of these mutants to growat the elevated temperature (Figure 9B). Because the mutatedprotein, gyp2 R295K is stably expressed (Figure 9C), these resultsprovide evidence that the GAP activity of Gyp2p is requiredto regulate Ypt31p function.

The GRAM domain is a protein module of $~$ 70 amino acids that hasbeen predicted to function as a protein- or lipid-binding motif(Doerks et al., 2000). In the sequences identified so far, aninvariable glycine residue in the GRAM domain (G80 in Gyp2p)has been proposed to be essential for function (Doerks et al.,2000). When gyp2 G80E is expressed in gyp2 ${Delta}$ trs130-HA^ts or gyp2 ${Delta}$ ypt32 ${Delta}$ ypt31-101^ts mutant cells, they were still able to growat the elevated temperature (Figure 9B), demonstrating thatan intact GRAM domain is required for Gyp2p regulation of Ypt31p.Mutation of this residue (G80E), while not affecting the stabilityof Gyp2p (Figure 9C), impaired the Ypt31p-GTPase activatingfunction of Gyp2p. The mechanism by which the GRAM motif participatesin the GAP function of Gyp2p is presently unclear. Our datado not preclude the possibility that the GRAM motif transientlyinteracts with a protein or lipid to regulate Gyp2p function(see Discussion).

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

A Role for Pik1p in Vesicular Transport
Previous work (Hama et al., 1999; Walch-Solimena and Novick,1999; Audhya et al., 2000) suggested that Pik1p-generated PtdIns(4)Pplays a direct role in the regulation of Golgi traffic and function.To date, the only identified component of a Pik1p-dependentsignaling pathway in yeast is Frq1p, a calcium-binding frequeninhomologue that directly activates Pik1p catalytic activity invitro (Hendricks et al., 1999). It is currently unclear whetherFrq1p regulates the pool of PtdIns(4)P that is relevant to vesiculartrafficking (Hendricks et al., 1999). To identify additionalsignaling pathway components of Pik1p, particularly those thatfunction together with Pik1p in Golgi-mediated vesicle trafficking,an SGA analysis utilizing a temperature-conditional pik1 mutantwas undertaken.

In this study, we report the first genome-wide SGA analysisof pik1. This approach identified genetic interactions uniqueto pik1, which both confirm an essential role for Pik1p in Golgi-dependenttrafficking and suggest a mechanistic involvement for Pik1pwith a specific subset of Golgi-associated proteins, includingthe Ypt31p rab-GTPase, the multicomponent TRAPPII protein complex,and the aminophospholipid translocase, Drs2p. We further showthat Pik1p and Ypt31p coordinately regulate traffic at the trans-Golgi,and that Ypt31p functions downstream of multiple TRAPPII components.On the basis of these genetic relationships, we were able tofurther elucidate the Ypt31p signaling pathway by identifyingGyp2p as a likely GAP for Ypt31p. From our SGA and phenotypicanalysis, we infer that a complex spatial and temporal interplayamong Pik1p, Ypt31p, TRAPPII and possibly additional traffickingcomponents converge to regulate Golgi secretory function.

Pik1p and Ypt31p Function Synergistically in Regulating Golgi Structure and Secretory Function
EM analysis demonstrated that pik1-139^ts (38°C), ypt32 ${Delta}$ ypt31-101^ts(38°C), and pik1-139^ts ypt31 ${Delta}$ double mutant cells (26°C)resulted in severe structural abnormalities of the Golgi (ourunpublished results). These results suggest that the concertedaction of Pik1p and Ypt31p was required to maintain the structuralintegrity and the unique membrane identity of the Golgi. Consistentwith a primary role in Golgi function, we demonstrate that bothPik1p and Ypt31p colocalize to Sec7p-enriched puncta, indicativeof trans-Golgi localization. Although the Golgi in pik1-139^tsypt31 ${Delta}$ double mutant cells remains remarkably competent in the processingof several cargoes (CPY, Gas1p) and the traffic of several plasmamembrane resident proteins (Tat2p, Hxt1p), we found that thecollaborative function of Pik1p and Ypt31p was required forthe targeting of two proteins, the yeast SNARE Snc1p and thecell wall enzyme Chs3p to sites of polarized growth and membranefusion (i.e., growing bud or septum). Snc1p and Chs3p are distinctfrom other transport cargoes in yeast, as they require continualrecycling via early endosomes to maintain their proper subcellularlocalization (Lewis et al., 2000; Valdivia et al., 2002). Hence,the molecular components involved in the efficient recyclingof Snc1p and Chs3p are starting to emerge, and our data suggestthat Pik1p and Ypt31p activities are particularly importantfor this trafficking pathway (Figure 10A).

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Figure 10. (A) Snc1p trafficking to the plasma membrane (PM) in yeast requires Golgi and early endosome (EE) function. Inactiva