Pga1 Is an Essential Component of Glycosylphosphatidylinositol-Mannosyltransferase II of Saccharomyces cerevisiae

Keisuke Sato, Yoichi Noda, and Koji Yoda

Department of Biotechnology, University of Tokyo, Tokyo 113-8657, Japan

Submitted March 19, 2007; Revised June 21, 2007; Accepted June 22, 2007
Monitoring Editor: Akihiko Nakano

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The Saccharomyces cerevisiae essential gene YNL158w/PGA1 encodesan endoplasmic reticulum (ER)-localized membrane protein. Weconstructed temperature-sensitive alleles of PGA1 by error-pronepolymerase chain reaction mutagenesis to explore its biologicalrole. Pulse-chase experiments revealed that the pga1^ts mutantsaccumulated the ER-form precursor of Gas1 protein at the restrictivetemperature. Transport of invertase and carboxypeptidase Y werenot affected. Triton X-114 phase separation and [³H]inositollabeling indicated that the glycosylphosphatidylinositol (GPI)-anchoringwas defective in the pga1^ts mutants, suggesting that Pga1 isinvolved in GPI synthesis or its transfer to target proteins.We found GPI18, which was recently reported to encode GPI-mannosyltransferaseII (GPI-MT II), as a high-copy suppressor of the temperaturesensitivity of pga1^ts. Both Gpi18 and Pga1 were detected inthe ER by immunofluorescence, and they were coprecipitated fromthe Triton X-100–solubilized membrane. The gpi18^ts andpga1^ts mutants accumulated the same GPI synthetic intermediateat the restrictive temperature. From these results, we concludedthat Pga1 is an additional essential component of the yeastGPI-MT II.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many proteins synthesized at the surface of the endoplasmicreticulum (ER) are transported through the secretory pathwayto proper locations in the cell where they function (Palade,1975; Mellman and Warren, 2000). The ER is an organelle wherethe major secretory pathway starts, and the folding status ofthe proteins are monitored to pass this pathway (Kleizen andBraakman, 2004). In the ER, several modifications are performedon the proteins, such as N-glycosylation, O-glycosylation, andglycosylphosphatidylinositol (GPI)-anchoring (Sipos and Fuller,2002). The GPI is a complex glycolipid with a core structure,phosphoethanolamine (EtN-P)-6-mannose (Man)- ${alpha}$ 1,2-Man- ${alpha}$ 1,6-Man- ${alpha}$ 1,4-glucosamine(GlcN)- ${alpha}$ 1,6-inositol-phospholipid, that is conserved in all eukaryoticcells (Kinoshita and Inoue, 2000) and functions as a membraneanchor for many cell surface proteins (Englund, 1993). In buddingyeast Saccharomyces cerevisiae, GPI synthesis and GPI-anchoringare carried out by >20 gene products, and most of the genesare essential for cell viability (Pittet and Conzelmann, 2006).Many GPI-anchored proteins lose lipid moiety at a certain stageof maturation, and they become attached to the cell wall $beta$ 1,6-glucanthrough the remaining mannose residues, contributing to thecell wall integrity (Lu et al., 1995). Construction and attachmentto the target protein of GPI are carried out on the ER membrane.The GPI is synthesized by a stepwise addition of sugars, anacyl chain, and EtN-P to phosphatidylinositol (PI). The GPItransamidase complex removes the C-terminal GPI attachment signalpeptide of the target protein and links the newly generatedC-terminal end to the EtN-P of the complete GPI precursor lipid(Eisenhaber et al., 2003). All of the genes that are known tobe involved in GPI synthesis and GPI-anchoring in S. cerevisiaehave homologues in mammals. Moreover, GPI is essential for theviability of some protozoan species, such as Leishmania mexicanaand the bloodstream form of Trypanosoma brucei. It has beensuggested that the pathway of GPI synthesis is mostly conservedamong the species; thus, S. cerevisiae can contribute to GPIresearch as a model organism.

The GPI of S. cerevisiae contains four Man residues. The fourthMan has essential roles because SMP3, which encodes the enzymeto add the fourth Man, is essential for viability (Grimme etal., 2001), although the addition of fourth Man is not essentialand the GPIs contain only three Man residues in other organisms(Taron et al., 2004). The enzymes that add Man to GPI precursorsare called GPI-mannosyltransferase (GPI-MT) I, -II, -III, and-IV, according to the order of mannose addition. Each GPI-MTconsists of at least one protein with several transmembranedomains that has homology to other enzymes responsible for glycosylation(Takahashi et al., 1996; Grimme et al., 2001; Maeda et al.,2001; Ashida et al., 2005; Fabre et al., 2005; Kang et al.,2005). So far, GPI-MT I has been the only enzyme that is foundto consist of multisubunits. Gpi18 is recently reported to berequired for the addition of a second Man to the GPI precursor,and its mammalian homologue PIG-V acts as GPI-MT II in Chinesehamster ovary (CHO) cells. PIG-V could partially rescue thelethality of ${Delta}$ gpi18 cells (Fabre et al., 2005; Kang et al., 2005).

Recently, large-scale analyses of the essential genes of S.cerevisiae were reported from several laboratories (Hazbun etal., 2003; Mnaimneh et al., 2004; Davierwala et al., 2005; Schuldineret al., 2005). In their analyses, target genes were placed underthe control of regulatable promoters, and the physiologicalroles of encoded proteins were predicted by the phenotypes theyshowed under the expression shut-off, and, in some cases, bythe synthetic sickness or lethality with other genes that encodeproteins with known functions. Although these approaches provedto be very useful for dealing with many genes, and they suggestedpossible involvement of the given gene product in a certainbiological pathway, the functional and mechanistic informationobtained for each gene product seemed to be sometimes limited.So, we took a different approach to find proteins that executeundefined but essential roles in the ER. We created the temperature-sensitive(ts) mutants of essential genes that encode the ER-localizedproteins by error-prone polymerase chain reaction (PCR). Theadvantage of using ts mutants is that they often display thephenotypes immediately after the temperature shift; they sometimesdisplay allele-specific phenotypes useful for regional analyses;and they are suitable for screening genetic interactions, especiallygenes that function as multicopy suppressors, which often providewith very valuable clues to characterize the protein function.The ER-localized proteins were selected from membrane proteinsencoded by essential genes by observing the localization ofthe green fluorescent protein (GFP)-fusion proteins. One ofthem, YNL158w/PGA1, encodes a protein that has no similaritywith mammalian proteins, and it was reported to be requiredfor the proper processing of Gas1 (a GPI-anchored protein ofthe plasma membrane) and Pho8 (an alkaline phosphatase in thevacuole); therefore, Pga1 has been suggested to be importantfor normal ER function (Davierwala et al., 2005). Here, we showthat Pga1 is an essential component of GPI-MT II. We identifiedGPI18 as a high-copy suppressor of pga1^ts, and further characterizationindicated that Pga1 is responsible for the second mannose additionto GPI precursors as a partner of Gpi18. This is the first reportto show that a gene with no mammalian homologue is involvedin GPI synthesis in S. cerevisiae.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Strains and Media
S. cerevisiae strains used in this study are listed in Table 1.They were grown in YPD (1% Bacto yeast extract [BD Biosciences,Franklin Lakes, NJ], 2% Bacto peptone [BD Biosciences], and2% glucose) or SD (0.17% yeast nitrogen base without amino acids[BD Biosciences], 0.5% ammonium sulfate, 2% glucose, and appropriatesupplements) medium at 30°C unless other temperatures wereindicated. An SG (2% galactose instead of glucose in SD) mediumwas used to induce genes under GAL1 promoter. Ammonium sulfatewas replaced with ammonium chloride in the low-sulfate SD medium.Solid media were made with 1.5% agar; 20 µg/ml each ofhistidine, tryptophan, and uracil and 0.1% 5-fluoroorotic acid(Sigma-Aldrich, St. Louis, MO) were added in SD to make a 5-fluorooroticacid (5-FOA) plate for Ura3⁺ counterselection, and 20 µg/mlphloxine B (Sigma-Aldrich) was added in YPD to make a phloxineplate (Tsukada and Ohsumi, 1993) for selection of temperature-sensitivemutants. Escherichia coli DH5 ${alpha}$ (F^–, supE44 ${Delta}$ lacU169 ${varphi}$ 80lacZ ${Delta}$ M15hsdR17 recA1 endA1 gyrA96 thi-1 relA1) was used in plasmid propagation.E. coli was grown in an LB (1% Bacto tryptone [BD Biosciences],0.5% Bacto yeast extract [BD Biosciences]) and 0.5% NaCl) medium.

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Table 1. S. cerevisiae strains used in this study

Plasmid Construction
Primers used in this study are listed in Table 2. The nucleotidesequence of each amplified fragment was confirmed.

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Table 2. Primers used in this study

Low-copy PGA1 expression plasmid (pCA148 or pKS38) was madeby ligation of the PCR amplification fragment from the genomicDNA by using the primers CA177 and CA178 into the plasmid pRS316or pRS313, respectively. Low-copy GPI18 expression plasmid (pKS71)was made by ligation of the PCR amplification fragment fromthe genomic DNA by using the primers KS52 and KS53 into theplasmid pRS316. High-copy GPI18 expression plasmid (pKS72) wasmade by replacing the plasmid vector with pRS426. High-copyGPI14, PBN1, GPI10, or SMP3 expression plasmid (pKS97, pKS98,pKS96, or pKS99, respectively) was made by ligation of the PCRamplification fragment from the genomic DNA by using the primers(KS59 and KS60, KS61 and KS62, KS57 and KS58, or KS63 and KS64,respectively) into the plasmid pRS426. The C-terminal taggingof GFP to Pga1 (pKS5) was made by ligation of the PCR amplificationfragment from the genomic DNA by using the primers CA159 andYN209 into the plasmid pRS316-GFP-TDH1 terminator (pCA42).

The C-terminal fusion of 6myc to Pga1 (pKS22 or pKS110) wasmade by replacing the vector of the plasmid pKS5 with pNT125-2(pRS316-6myc-TDH1 terminator) or pKS55 (pRS313-6myc-TDH1 terminator),respectively. The N-terminal fusion of GFP to Gpi18 (pKS128)was made by ligation of the PCR amplification fragment fromthe genomic DNA by using the primers KS65 and KS53 into theplasmid pRS316-YPT1 promoter-GFP (pCA42). The plasmid pKS213for gap repair used to construct pga1^ts mutants was made asfollows: the PCR amplification fragment from the genomic DNAusing primers CA159 and KS5 was ligated into pRS313, and thenanother PCR amplification fragment from the genomic DNA usingprimers KS6 and CA160 was ligated into the newly generated plasmid.The plasmid pKS170 for gap repair used to construct gpi18^tsmutants was made as follows: the PCR amplification fragmentfrom the genomic DNA using the primers KS52 and KS85 was ligatedinto pRS313 and then another PCR amplification fragment fromthe genomic DNA using the primers KS86 and KS53 was ligatedinto the newly generated plasmid. Plasmid pAK35 or pKS81 usedfor the integration of pga1^ts alleles to the yeast chromosomewas made by insertion of the DNA fragment containing the encodingORF and its downstream sequence from pKSTS16 or pKSTS15 to pTY23(pBluescript SK⁺-LEU2) and following insertion of the PCR amplificationfragment from the genomic DNA using the primers KS54 and CA160.Plasmid pKS188 or pKS195 for the integration of the gpi18^tsallele to the yeast chromosome was made by insertion of thePCR amplification fragment from the genomic DNA using the primersKS83 and KS85 into pTY23 and following insertion of the DNAfragment containing encoding open reading frame (ORF) and itsdownstream sequence from pKSTS113 or pKSTS114. The plasmid pKS173for integration of GPI18 expressing under the control of GAL1promoter was made as follows. A DNA fragment containing GAL1promoter from pYES2 was inserted into pTY23, and the PCR amplificationfragment from the genomic DNA using the primers KS65 and KS53was ligated into the newly generated plasmid behind the LEU2gene. The plasmid pKS189 for the integration of PGA1 expressingunder the control of GAL1 promoter to the chromosome was madeas follows: a DNA fragment containing GAL1 promoter from pYES2was inserted into pTY23, and the PCR amplification fragmentfrom the genomic DNA using the primers CA186 and CA160 was ligatedinto the newly generated plasmid behind the LEU2 gene.

Antibodies
Antisera against Scs2 and Kar2 were kindly provided by Dr. S.Kagiwada (Nara Woman's University, Japan) and Dr. Masao Tokunaga(Kagoshima University, Japan), respectively. Anti-3-phosphoglyceratekinase mouse (anti-PGK, 22C5; Invitrogen, Carlsbad, CA), anti-mycmouse (9E10; Berkeley Antibody, Richmond, CA), anti-alkalinephosphatase (ALP) mouse (1D3; Invitrogen) and monoclonal antibodies(mAbs), and anti-carboxypeptidase Y rabbit (anti-CPY; Rockland,Gilbertsville, PA) polyclonal antibody were purchased. The anti-GFPantiserum was prepared by immunizing rabbits with the glutathioneS-transferase-GFP fusion protein as the antigen. For Westernblotting, these antisera were diluted at 1:1000.

Construction of Temperature-sensitive Mutant Alleles of PGA1 and GPI18
The DNA fragment containing the whole PGA1 gene with the authenticpromoter and terminator was amplified using primers KS159 andKS160 under an error-prone PCR condition (Muhlrad et al., 1992).KSY33 was transformed with the mixture of the amplified fragmentand the EcoRI-cleaved pKS213 to integrate fragments into theplasmid by gap repair. The His⁺ transformants were replicatedto 5-FOA plates to remove pKS5, and then they were replicatedto phloxine B plates and incubated at 37°C for 2 d. Thecells that formed pink colonies were tested for single colonyformation at 25 and 37°C. After confirming that the temperaturesensitivity was due to the plasmid, the nucleotide sequencesof the mutant pga1 were determined. Construction of the ts mutantalleles of GPI18 was performed almost the same way as describedabove, except that primers KS52 and KS53 were used, the gaprepair plasmid was the SmaI-cleaved pKS170, and the transformedstrain was KSY239.

Subcellular Fractionation and Solubility Test of Membrane Proteins
Cells were converted to spheroplasts and burst in B88 (20 mMHEPES, pH 6.8, 150 mM potassium acetate, 5 mM magnesium acetate,and 200 mM sorbitol) containing protease inhibitors (1 µg/mleach of chymostatin, aprotinin, leupeptin, pepstatin A, antipain,and 1 mM phenylmethylsulfonyl fluoride). Unbroken cells wereremoved by centrifugation at 1000 x g for 5 min. For subcellularfractionation, the cleared lysate was sequentially centrifugedto generate 10,000 x g pellet (P10), 100,000 x g pellet (P100),and 100,000 x g supernatant (S100). Each fraction was adjustedto the original volume of the lysate and the same amount wasapplied for SDS-polyacrylamide gel electrophoresis (PAGE) andWestern blotting. As a solubility test, a portion of lysatewas mixed with the same amount of B88 containing 2% Triton X-100,2 M NaCl, 0.2 M Na₂CO₃, or 4 M urea, and the mixture was kepton ice for 15 min. After removing a sample as the total, themixture was centrifuged at 100,000 x g for 60 min. The precipitatewas suspended in the same volume of the same buffer as the supernatant.

BiP Secretion Blots
The secretion of lumenal ER proteins was analyzed as describedpreviously (Lewis et al., 1997).

Triton X-114 Phase Separation
The Triton X-114 phase separation was performed essentiallyas described by Doering and Schekman (1996) with some modifications.In brief, the cells were incubated at 34°C for 12 h, collected,and disrupted with glass beads. After centrifugation at 1000x g for 5 min, the supernatant was incubated in B88 containing1% Triton X-114 on ice for 30 min. After the extract was centrifugedat 10,000 x g for 4 min at 4°C, the supernatant was keptat 32°C for 5 min and centrifuged at 13,000 x g for 30 sat room temperature to separate the detergent and aqueous phases.Each phase was re-extracted with either 1% Triton X-114 (finalconcentration) or buffer as appropriate. Each re-extracted phasewas subjected to SDS-PAGE, and Gas1, Scs2, or Pgk1 was detectedby Western blotting.

Indirect Immunofluorescence
Fixation and permeabilization of the yeast cells for indirectimmunofluorescence was performed as described by Wooding andPelham (1998), and subsequent steps were performed as describedby Vashist et al. (2002) with some modifications; a descriptionof the procedure is as follows. Log-phase cells grown at 30°Cwere fixed by adding 2.5 ml of fresh 10% paraformaldehyde to7.5 ml of yeast culture and pelleted by centrifugation. Theywere resuspended in 3.2 ml of PP (0.1 M potassium phosphate,pH 7.5), 1.8 ml of paraformaldehyde solution was added, andfixation was continued for an additional 15 min. Cells werethen washed four times in PP and resuspended in 1 ml of SPP(PP with 1.2 M sorbitol) containing 100 mM dithiothreitol. Tenmicroliters of lyticase was added, and incubation was continuedat 30°C. The spheroplasts were harvested by centrifugationand resuspended in 50 mM NH₄Cl in SPP, and then in SPP beforebeing transferred to polylysine-coated slides. The slides wereimmersed in methanol for 6 min and acetone for 30 s, both at–20°C, and then air-dried. The anti-myc mouse mAband the anti-Kar2 rabbit polyclonal antibody were diluted to1/40, 1/100 each in 1% skim milk, 0.1% bovine serum albumin,and 0.05% Tween 20 in Tris-buffered saline (TBS; 50 mM Tris,pH 7.4, and 150 mM NaCl), and incubations were carried out overnightat 4°C. Slides were washed and incubated in the secondaryantibodies (Alexa 488-conjugated goat antibody to mouse immunoglobulinG and Texas Red-conjugated goat antibody to rabbit immunoglobulinG) for 2 h at room temperature, washed with phosphate-bufferedsaline, and mounted as described by Kilmartin and Adams (1984).Images were obtained using an FV500 confocal laser-scanningmicroscope (Olympus, Tokyo, Japan).

Immunoprecipitation
Cells were grown at 30°C in SD medium to an OD_{600 nm} = 1.0,and 50 OD units of cells were converted to spheroplasts andburst in 1 ml of B88 containing protease inhibitors. Unbrokencells were removed by centrifugation at 1000 x g for 5 min.Then, 990 µl of the cleared lysate was mixed with 110µl of 10% Triton X-100 and kept on ice for 15 min. Themixture was centrifuged at 100,000 x g for 60 min. The supernatantwas recovered as the fraction "input." The rest of the supernatantwas mixed with anti-myc monoclonal (9E10) antibody and keptgently rotating at 4°C for 1 h. Protein A-Sepharose beads(GE Healthcare, Little Chalfont, Buckinghamshire, United Kingdom)washed with B88 containing 1% Triton X-100 were added and incubationwas continued at 4°C for 1 h further. The mixture was centrifugedat 1000 x g for 5 min, and the supernatant was recovered asthe fraction "unbound." The beads were washed 4 times with B88containing 1% Triton X-100 and then washed with 1 ml of 5 mMammonium acetate. The bound proteins were eluted with 50 µlof 0.5 M acetic acid/ammonium acetate, pH 3.4, and recoveredas the fraction "bound." The same volume of each fraction wassubjected to the SDS-PAGE, and the indicated proteins were detectedby Western blotting.

Invertase Detection
Cells were incubated in YPD to OD_{600 nm} = 1.0 at 25°C, and10 OD unit of cells were shifted to 25 or 37°C, and incubationwas continued for 30 min. Cells were washed in YPS (2% sucroseinstead of glucose in YPD) and incubated in YPS for 3 h at thesame temperature as they were incubated before, after whichcells were collected and resuspended in solution A (25 mM Tris,pH 8.0, 0.6 M sorbitol, 2.5 mM sodium azide, 0.1% $beta$ -mercaptoethanol,and 0.25 mg/ml Zymolyase [Zymo Research, Orange, CA]). After37°C incubation for 30 min, the mixture was centrifugedat 13,400 x g for 10 min at 4°C, and the supernatant wassubjected to native PAGE. Secretory invertase in the gel wasdetected by activity staining as described by Ballou (1990).

Pulse-Chase Experiments of CPY and Gas1
Yeast strains were grown at 25°C in low-sulfate SD to OD_600nm = 1.0. Two and a half OD units of cells were harvested bycentrifugation and resuspended in 100 µl of SD lackingsulfate. Pulse labeling was initiated 30 min after the shiftto the restrictive temperature of 37°C by the addition of50 µCi of Tran[³⁵S]-label (MP Biomedicals, Irvine, CA).After 5 min of pulse labeling, the chase period was initiatedby the addition of prewarmed 500 µl of chase solution(SD with 0.5% casamino acids [BD Biosciences]) and terminatedby transferring the cells to a tube on ice containing 100 µlof 60 mM sodium azide. After a minimum of 10 min on ice, thecells were collected and broken by vortexing with glass beadsin TBS containing 1% SDS and protease inhibitors, and then theywere boiled for 5 min. The boiled mixture was added with 4 volumesof TBS containing 2% Triton X-100, and centrifuged at 15,000x g for 5 min. The supernatant was added with anti-CPY or anti-Gas1antibody, and then it was rotated overnight. Protein A-Sepharosewashed with B88 containing 1% Triton X-100 was added to themixture and rotated for 1 h. Recovered protein A-Sepharose waswashed in TBS containing 1% Triton X-100 5 times. Immunoprecipitatedproteins were eluted by boiling in SDS-PAGE sample buffer for5 min and resolved by SDS-PAGE through 7.5% gel. ³⁵S-labeledCPY or Gas1 was detected by autoradiography and analyzed byBAS-3000 (Fuji Film, Tokyo, Japan).

Radiolabeling of Lipids with myo-2-[³H]Inositol
For myo-2-[³H]inositol labeling of temperature-sensitive strains,cultures of each strain were grown at 25°C in SD mediumto an OD_{600 nm} = 1.0, and 10 OD units of cells were washed twicein SD-inositol and then resuspended in 1 ml of SD-inositol.After incubation at 25°C for 30 min, these cultures wereshifted to 37°C for 20 min or maintained at 25°C before15 µCi of [³H]inositol (American Radiolabeled Chemicals,St. Louis, MO) was added to them, and radiolabeling was continuedfor 90 min at the same temperature. For [³H]inositol labelingof gpi18::LEU2-P_GAL1-GPI18 strains, cells were maintained onSG medium and then shifted to fresh SG or SD for 20 h to OD₆₀₀of $~$ 1. Ten OD cells were washed twice in SG-inositol or SD-inositol,resuspended in 1 ml of SG-inositol or SD-inositol, and thenincubated for 50 min at 30°C. After the incubation, 15 µCiof [³H]inositol was added to them, and radiolabeling was continuedfor 90 min at 30°C. To stop [³H]inositol labeling, NaN₃was added to a 10 mM final concentration each, and cells wereplaced on ice. Cells were collected by centrifugation, washedtwice in 10 mM NaN₃, and resuspended in 500 µl of CM extractionsolvent (CHCl₃/CH₃OH, 1:1, vol/vol). Glass beads (0.5 g) wereadded to the suspension, and cells were lysed by vortexing fourtimes for 1 min each. The lysate was spun at 15,000 x g for5 min, and the supernatant was collected and transferred toa new tube. Three hundred microliters of CMW (CHCl₃/CH₃OH/H₂O,10:10:3, vol/vol) was added to the remaining glass beads andcell debris, and the mixture was vortexed for 1 min. After centrifugation,supernatant was added to the first lipid extract. Pooled lipidswere dried in a speed-vac. The resulting pellet was resuspendedwith 150 µl of H₂O-saturated 1-butanol and extracted with75 µl of 1-butanol-saturated water. The organic phasewas collected, and the aqueous phase was backextracted withan additional 75 µl of H₂O-saturated 1-butanol. The pooledorganic phases were dried in a SpeedVac and resuspended in 30µl of CMW. All amounts of samples were loaded onto thinlayer chromatography (TLC) plates (Kieselgel 60; Merck, Darmstadt,Germany), developed in CHCl₃/CH₃OH/H₂O (5:5:1, vol/vol). TLC-separatedlipids were detected by autoradiography.

Radiolabeling of Proteins with myo-2-[³H]Inositol
Labeling of cells was performed as described above except forlabeling with 120 µCi of [³H]inositol for 2 h. Washedcells were resuspended in 200 µl of lysis buffer (50 mMTris-Cl, pH 6.8, 5 mM EDTA, pH 8.0, 1% SDS, 1% 2-melchaptoethanol,and protease inhibitors), and glass beads (0.2 g) were addedto the suspension. Cells were lysed by vortexing four timesfor 1 min each, placing the cells on ice between each vortexingcycle, and then boiled for 5 min. Four milliliters of Con Abuffer (50 mM Tris-Cl, pH 7.5, 1% Triton X-100, 500 mM NaCl,1 mM CaCl₂, 1 mM MgCl₂, and 1 mM MnCl₂) was added to the boiledsuspension, and the mixture was centrifuged at 15,000 x g. ConA-Sepharose (GE Healthcare) washed twice in Con A buffer wasadded to the supernatant and rotated overnight. Proteins wererecovered by boiling Con A-Sepharose in SDS-PAGE sample bufferfor 5 min, separated by SDS-PAGE through a 4–20% gradientgel (Daiichi, Tokyo, Japan), and then detected by autoradiography.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previously Uncharacterized Pga1 Protein Is an ER-resident Membrane Glycoprotein
We searched the Saccharomyces Genome Database (SGD) for essentialproteins with predicted transmembrane domain(s) to find proteinsthat execute essential functions in the ER. We introduced plasmidsconstructed to produce the GFP-fusion protein to each diploidstrain in which one of the alleles was replaced by kanMX4. Ahaploid deletion strain producing GFP-fusion protein was obtainedby tetrad analysis, and the localization of GFP was observedby fluorescent microscopy. We found that Ynl158w-GFP showedthe localization around the nucleus and at the cell periphery,which is a pattern common to the ER proteins (Figure 2A). YNL158w/PGA1is an essential gene and its gene disruptants were reportedto be inviable even under the laboratory culture conditions(Duenas et al., 1999). According to SGD, it encodes a 198 amino-acidpolypeptide of molecular weight = 22,383 and pI = 6.63, thebiochemical function of which remains unknown. Homologous sequenceswere found in several fungal genome databases by a FASTAP search(Figure 1A), but no homologues were found in the database ofhigher eukaryotes. The hydropathy plot indicated that thereare two hydrophobic segments at the N and C termini (Figure 1B).SignalP predicted the N-terminal segment functions as the signalpeptide. The sequence ²³Ala-Asn is the most probable cleavagesite, and this cleavage finally generates a polypeptide of 175amino-acid residues.

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Figure 1. Sequence alignment of Pga1 protein and its homologues and the hydropathy profile of Pga1 protein. (A) Amino acid sequence alignment of the Pga1 homologues. Two hydrophobic segments are indicated by bars over the sequences, and the predicted signal peptide cleavage site is shown by an arrowhead. Nine terminal amino acids of the A. gossypii sequence were omitted to adjust the amino-acid alignment of the predicted signal peptides. The identical amino acids were highlighted with reverse letters. (B) The hydrophobicity index was calculated according to Kyte and Doolittle (1982)

, with a window size of 10 amino acids. Bold lines indicate the hydrophobic domains.

To confirm its localization to the ER, we fused 6myc at theC terminus of Pga1 and expressed it in ${Delta}$ pga1 cells, then we comparedits localization with the ER-marker Kar2 by indirect fluorescencewith confocal microscopy. The Pga1-6myc showed same patternas Pga1-GFP, and it colocalized with Kar2 (Figure 2A). Next,we performed biochemical analysis of the Pga1-6myc. The Pga1-6mycwas detected by immunoblotting, by using the anti-myc antibodyas a main band of 41 kDa. By differential centrifugation ofthe cell lysate, Pga1-6myc was recovered mainly in the P10 fractionand some in the P100 fraction, but it was not detected in thesoluble S100 fraction (Figure 2B). The ER membrane protein Scs2was similarly recovered as Pga1, whereas the early Golgi markerVan1 was recovered almost evenly in P10 and P100 fraction, andthe late Golgi marker Kex2 was mainly recovered in P100 fraction.Together with the results of microscopy observation, Pga1 shouldbe the ER-localized protein. Next, we tested whether Pga1 isactually integral to the ER membrane. As shown in Figure 2C,Pga1-6myc was recovered in the precipitate even in the presenceof 1 M sodium chloride, 0.1 M sodium carbonate, pH 11, or 2M urea, but it became soluble in the presence of 1% Triton X-100.Therefore, we concluded that Pga1 is integral to the ER membrane.

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Figure 2. Pga1 localizes in the ER as a glycosylated integral membrane protein. Pga1-GFP or Pga1-6myc was produced from CEN plasmid in ${Delta}$ pga1 cells, KSY33 or KSY63. (A) Confocal microscopic observation of Pga1-GFP and Pga1-6myc. The immunofluorescence images of the ER-marker Kar2 protein and the merged images with Pga1-6myc are also shown. (B) Subcellular fractionation of Pga1-6myc, the ER-marker Scs2, the early Golgi marker Van1, and the late Golgi marker Kex2. (C) Pga1-6myc and the ER membrane protein Scs2 were subjected to the solubilization test by using 1 M NaCl, 0.1 M Na₂CO₃, 2 M urea, and 1% Triton X-100. (D) The molecular mass of Pga1p-6myc before (–) and after (+) endoglycosidase H treatment was determined by SDS-PAGE and Western blotting.

There are two potential N-glycosylation sites, ⁷²Asn-Thr-Thrand ⁸⁰Asn-Thr-Thr, in the hydrophilic region of Pga1 polypeptide.To obtain topological information, we examined the effect ofendoglycosidase H (endoH) treatment on Pga1-6myc. As shown inFigure 2D, a 41-kDa band disappeared and a 36-kDa band appearedafter endoH digestion. Therefore, Pga1 accepted N-glycosylation,which indicates that the hydrophilic domain localizes in thelumen of the ER. Cells expressing Pga1 tagged with 6myc at itsN terminus (6myc-Pga1) accumulated 6myc-Pga1 whose mobilityof SDS-PAGE was not affected by endoH treatment (data not shown),which may indicate that N-terminal tagging to Pga1 disturbedtranslocation to the ER lumen. This is consistent with the SignalPprediction that the N-terminal hydrophobic segment of Pga1 functionsas a signal peptide.

Isolation of Mutants with Temperature-sensitive Alleles of PGA1
Next, we sought to create temperature-sensitive alleles of PGA1by error-prone PCR mutagenesis to investigate the biologicalrole of Pga1. We obtained three mutant PGA1 plasmids [pKSTS16(pga1-1), pKSTS13 (pga1-2), and pKSTS15 (pga1-3)], which supportedgrowth of the ${Delta}$ pga1 haploid strain at 25°C, but not at 37°C.Nucleotide sequences indicated that a number of amino acid substitutionsoccurred in each of the mutant alleles. The amino acid substitutionsin the pga1-1 mutation were F20I, M64T, T74P, D75G, I107F, N111S,T126A, Y144H, P152S, and Y169H; those in pga1-2 were F36Y, I57T,Y95C, C100Y, and N110S; and those in pga1-3 were T74A, D92G,W101R, I107V, Q113R, T121A, T136A, N192S, L196P, and K197E.These substitutions collectively contributed to the mutant phenotype,because the reversion of some residues resulted in the lossof temperature sensitivity, but these residues alone did notgive temperature sensitivity. The chromosomal wild-type PGA1allele was replaced with the mutant allele pga1-1 or pga1-3by homologous recombination for further analysis.

Characterization of pga1^ts Mutants
Localization in the ER suggested that Pga1 has an essentialrole involved in the phenomenon that specifically occurs inthe ER. Therefore, we examined whether translocation, modification,and/or transport of secretory proteins was affected in thesepga1 mutants. The process of protein transport was analyzedby pulse-chase experiments of Gas1 (Nuoffer at al., 1993; Popoloand Vai, 1999) and CPY (Van Den Hazel et al., 1996). A GPI-anchoredplasma membrane protein Gas1 enters in the ER accompanied withthe cleavage of the N-terminal secretion signal peptide, andcore glycosylation of its N- and O-carbohydrate modificationsites, and it becomes the 105-kDa ER form proGas1 (Kodukulaet al., 1993). Then, the proGas1 C-terminal hydrophobic signalpeptide is replaced with the GPI-anchor. This GPI-anchored proGas1is transported to the plasma membrane through the Golgi whereit receives the further addition of carbohydrates to the glycosylchains, and becomes the 125-kDa mature form. ProCPY receivescore N-glycosylation in the ER (form p1), additional glycosylationin the Golgi (form p2), and finally it becomes the mature enzyme(form m) by the removal of propeptide in the vacuole. As shownin Figure 3A, the 105-kDa precursor of Gas1 was largely convertedto the mature 125-kDa form during a 30-min chase in the wildtype both at 25 and 37°C. In the pga1-1 mutant, the matureform appeared at 25°C but not at 37°C. A large amountof the ER-form Gas1 precursor accumulated at 37°C and onlya faint signal of the mature form appeared after the 30-minchase. In the sec12-ts mutant defective in the formation ofCOPII transport vesicles also failed to produce the mature-formGas1 at 37°C and accumulated a precursor with somewhat reducedelectrophoretic mobility. In contrast, the transport of CPYnormally occurred in the pga1-1 mutant both at 25 and 37°C,whereas the sec12-ts mutant accumulated the ER-form precursorof CPY (Novick et al., 1980). These results suggest that Pga1has an essential role in the processing or transport of a GPI-anchoredmembrane protein Gas1 but not in those of a soluble vacuolarprotein CPY. Secretion and N-glycosylation of the periplasmicinvertase were normal in the pga1-1 mutant (Figure 3B; Novicket al., 1980). The O-glycosylation of the extracellular Kre9(Lussier et al., 1995) was also normal in the pga1-1 mutant(data not shown). The retention system of the ER lumenal proteins(Lewis et al., 1997) was normal, because no leakage of Kar2in the medium was detected (Figure 3C). ProALP is also transportedthrough the Golgi to the vacuole but without passing the endosome,and the propeptide is removed in the vacuole (Klinosky and Emr,1989). An accumulation of soluble-form ALP was found in thepga1-1 mutant (Figure 3D), which is consistent with the observationin the previous report (Davierwala et al., 2005). Because thesec12^ts cells also showed similar accumulation of soluble-formALP at the permissive temperature, this might be a consequenceof some aberrant condition in the ER.

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Figure 3. The secretion-related characteristics of the temperature-sensitive pga1-1 mutant. (A) The transport of CPY and Gas1 from the ER in the pga1-1 cells was analyzed by a pulse-chase experiment at either 25 or 37°C. Proteins were pulse labeled with Tran[³⁵S]-label for 5 min and chased for indicated times. The immunoprecipitated CPY and Gas1 were detected by SDS-PAGE and autoradiography. ER, the ER-form proGas1(105 kDa); Golgi, the Golgi-form Gas1(125 kDa); p1, precursor CPY in the ER; p2, precursor CPY in the Golgi; m, mature CPY in the vacuole. (B) The N-glycosylation of secretory invertase in the pga1-1 cells at either 25 or 37°C was analyzed by native PAGE and activity staining. (C) The leakage of Kar2 protein (BiP) to the medium in the wild-type (WT), ${Delta}$ erd1, ${Delta}$ pga1/PGA1 and pga1-1 cells was analyzed at 25°C by membrane filter trapping and immunological detection of BiP. (D) The processing of ALP precursor in the WT, sec12^ts, and pga1-1 cells at either 25 or 37°C was analyzed by SDS-PAGE and Western blotting. p, precursor (ER) form; m, mature (vacuolar) form; s, soluble form of ALP.

The proGas1 Protein Accumulated in pga1^ts Mutants Is Not GPI-Anchored
Accumulation of proGas1 in the ER might result from either oftwo deficiencies. First, because GPI-anchor attachment is requiredfor the exit of the GPI target proteins from the ER (Nuofferet al., 1993

; Doering and Schekman, 1996

), a failure to produceor attach GPI would result in proGas1 accumulation. Second,mutants specifically defective in the transport of GPI-anchoredproteins also accumulate 105-kDa Gas1. Because the GPI-anchored105-kDa Gas1 protein is transported to the Golgi via COPII vesiclewith the assistance of p24-family proteins Emp24 and Erv25 (Munizet al., 2000

; Belden and Barlowe, 2001

), in the ${Delta}$ emp24 mutantcell, the exit of Gas1 from the ER is delayed and the 105-kDaGas1 precursor accumulates. To determine which deficiency causedthe defect of Gas1 processing observed in the pga1-1 mutant,the proteins were subjected to Triton X-114 phase separationthat distinguishes hydrophobicity (Doering and Schekman, 1996

).Cells were grown at the semipermissive temperature for the pga1-1mutant (34°C) for 12 h. The 105-kDa band, which representsthe precursor form of Gas1 in the ER was only faintly detectedin the total sample of the wild-type cell (Figure 4A, lane 1),but the amount significantly increased in the ${Delta}$ emp24 and pga1-1mutant cells (Figure 4A, lanes 4 and 7). In the pga1-1 mutantcells, a significant amount of 125-kDa band that representsthe mature form of Gas1 was detected, probably because the mutantPga1-1 was not completely inactive in this condition; however,the 105-kDa band was more abundant than the 125-kDa band. GPIattachment increases the hydrophobicity of target proteins andis known to cause an increase of the amount of target proteinsrecovered in the detergent phase when separated with TritonX-114. Consistent with our prediction, the 125-kDa Gas1 in eachcell and the 105-kDa Gas1 accumulated in the ${Delta}$ emp24 mutant wasmainly detected in detergent phase, indicating these Gas1 wereGPI-anchored (Figure 4A, lanes 3, 6, and 9). In contrast, theER-form of Gas1 accumulated in pga1-1 cells was mainly detectedin the aqueous phase (Figure 4A, lane 8). So, the 105-kDa Gas1in the pga1-1 mutant cell was suggested to represent the Gas1that was not GPI-anchored.

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Figure 4. The pga1-1 mutant showed temperature-sensitive defects in the GPI-anchoring of Gas1 and other GPI-anchored proteins. (A) Cleared lysate (total, T) of the WT, ${Delta}$ emp24, and pga1-1 cells was treated with 1% Triton X-114 and separated into the aqueous (A) and detergent (D) phases. Gas1, integral ER membrane protein Scs2 and the cytosolic 3-phosphoglycerate kinase (Pgk1) were detected by SDS-PAGE and Western blotting. (B) Cells were metabolically labeled with [³H]inositol and glycoproteins were collected using Con A-Sepharose. The wild-type (lanes 1 and 2) and pga1-1 (lanes 3 and 4) cells were grown at either 25°C (lanes 1 and 3) or 37°C (lanes 2 and 4). The concentrated glycoproteins were resolved by SDS-PAGE on 4–20% gradient gel and detected by Coomassie Brilliant Blue stain to confirm that the same amount of proteins was loaded on each lane. Lane M, molecular weight markers. (C) [³H]inositol incorporated into the glycoproteins was detected by autoradiography of the same gel. Lanes were the same as in B.

Because all detectable protein-linked inositol in yeast is presentin the GPI-anchors, we can distinguish whether the GPIs wereattached to its target proteins by checking the inositol incorporationto proteins. Therefore, we metabolically labeled the cell with[³H]inositol, and we analyzed the total protein for modificationof the GPI-anchor to examine whether the pga1-1 mutant cellis actually defective in the GPI anchoring. Because all majorGPI-anchored proteins are glycoproteins, almost all inositol-incorporatedproteins can be recovered with Con A-Sepharose (Guillas et al.,2000

). As shown in Figure 4C, [³H]inositol was incorporatedin a number of proteins in the wild type, but a very small amountof [³H]inositol was detected in the pga1-1 mutant cells at 37°C.The equivalence of applied proteins was confirmed by CoomassieBrilliant Blue staining (Figure 4B). These results indicatedthat pga1-1 was defective in GPI synthesis or its anchoringto the target protein.

pga1^ts Mutants Display the Phenotypes Related to GPI-anchoring Defect
The mutants defective in GPI-anchoring generally show cell walldefects that are partially suppressed by increasing the osmolarityby adding 1 M sorbitol into the growth medium. Similarly, thepga1-1 mutant did not form colonies on the YPD plate at 36°Cfor 2 d, but the temperature sensitivity was partially suppressedby adding 1 M sorbitol to YPD (Figure 5A). At a sublethal temperature(34°C), a significant increase of the amount of Kar2p proteinin the ER lumen was found in the pga1-1 mutant (Figure 5B).This indicates the pga1 mutant induced the unfolded proteinresponse (UPR), which is commonly observed in GPI mutants (Nget al., 2000, Davydenko et al., 2005). In contrast, the ${Delta}$ emp24mutant that accumulates the ER-form Gas1 precursor due to thedefect in transport of GPI-anchored proteins from the ER doesnot show UPR induction, suggesting that the UPR is induced bythe accumulation of the GPI precursor or the target proteinwithout GPI-anchoring, but not by the accumulation of GPI-anchoredproteins. Mutants defective in GPI-anchoring are typically hypersensitiveto the chitin-binding dye Calcofluor White (CFW). At a permissivetemperature (30°C), the pga1-1 mutant showed a slightlyincreased sensitivity to CFW (Figure 5C). The ${Delta}$ gas1 mutant showedhigher sensitivity. These results strongly support the likelinessthat Pga1 is actually defective in GPI anchoring.

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Figure 5. The pga1-1 mutant displayed the phenotypes related to the defect of GPI-anchoring. (A) The temperature sensitivity of pga1-1 was partially suppressed by high osmolarity. The WT and pga1-1 mutant were streaked on YPD with or without 1 M sorbitol and grown 2 d at 36°C. (B) Unfolded protein response was induced in pga1-1 mutant cells. The amount of Kar2 protein (BiP) in the WT, pga1-1 mutant and ${Delta}$ emp24 mutant grown at 34°C was analyzed by SDS-PAGE and Western blotting, by using the ER membrane protein Scs2 as the loading control. (C) The pga1-1 mutant showed increased sensitivity to Calcofluor white. Ten microliters of 10-fold serially diluted suspension of the WT, ${Delta}$ gas1, and pga1-1 mutant cells were spotted on SD agar with or without 40 µg/ml Calcofluor White, and then the cells were incubated for 2 d at 30°C.

Interaction of Pga1 with Gpi18, an Essential Glycosylphosphatidylinositol-Mannosyltransferase II Component
The defect of GPI anchoring in the pga1-1 mutant strongly suggestedthe involvement of PGA1 in GPI synthesis or anchoring process,but there are many steps in GPI synthesis and its anchoringto the target proteins. To determine where Pga1 functions inthe pathway, we screened for the multicopy suppressor genesof the temperature sensitivity of the pga1-1 mutant, becauseit often becomes an effective clue to elucidate the functionalrole of uncharacterized gene products. We introduced the 2µplasmid library to the pga1-1 mutant cells and sought the colonieswhose viability at 37°C were dependent on the introducedplasmids. As a result, we found that the GPI18 gene could recoverthe growth defect of the pga1-1 mutant at 37°C by its introductionon 2µ plasmid (Figure 6A). GPI18 was recently reportedto encode GPI-MT-II (Fabre et al., 2005

; Kang et al., 2005

).GPI-MT-II transfers the second Man from dolichol-P-Man to theMan-GlcN-PI precursor in the GPI anchor, so we supposed thatPga1 would have a function related to mannosylation in GPI synthesis.To test the possibility that Pga1 has genetic interaction withother GPI-MTs, we introduced GPI14, PBN1, GPI10, or SMP3 on2µ plasmid. GPI14 and PBN1 encode subunits of GPI-MT-I(Maeda et al., 2001

; Ashida et al., 2005

), GPI10 encodes thethird ${alpha}$ 1,2-mannosyltransferase, and SMP3 encodes the last ${alpha}$ 1,2-mannosyltransferase(Grimme et al., 2001

). However, multicopy expression of eachgene could not restore the growth of the pga1-1 mutant at 37°C(Figure 6B). The multicopy GPI18 could not suppress the lethalityof the ${Delta}$ pga1 null mutant (Figure 6C), indicating that Pga1 hasan indispensable role related to GPI18.

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Figure 6. Temperature sensitivity of the mutants of PGA1 and GPI18 was suppressed by introducing the mutual multicopy gene. (A) The colony-forming activity at 37°C of pga1-1 mutant was recovered by the GPI18 gene on the 2µ plasmid and that of gpi18–6 mutant was recovered by the PGA1 gene on the 2µ plasmid. (B) The high-copy introduction of GPI14, PBN1, GPI10, or SMP3 genes responsible for mannosylation in the yeast GPI synthesis did not suppress temperature sensitivity of the pga1-1 mutant at 37°C. (C) The heterozygous PGA1/ ${Delta}$ pga1::kanMX4 diploid cells were transformed with the CEN-PGA1 (top) or 2µ-GPI18 (bottom) plasmid, and then they were sporulated. The spores were dissected to assess the complementation by tetrad analysis.

Because only GPI18 could rescue the growth defects of pga1-1mutant cells, but other genes encoding GPI-MTs could not, thespecific association between PGA1 and GPI18 was indicated. Therefore,we investigated the interaction of the two proteins in yeastcells. For this purpose, PGA1-6myc and GFP-GPI18 on low-copyplasmids were expressed in ${Delta}$ pga1 cells. The fluorescent imagingusing GFP-tagged Gpi18 and Pga1-6myc indicated that both proteinsmainly localized to the ER, and the merged images indicatedthat the two proteins were in the same compartments in the ER(Figure 7A). GFP-Gpi18 was mainly recovered in the P10 fractionby subcellular fractionation (Figure 7B), and it was only solubilizedby Triton X-100 by our solubilization test (Figure 7C), whichindicates that Gpi18 is an integral ER membrane protein. Toexamine whether there is a physical protein–protein interactionbetween Gpi18 and Pga1, we conducted immunoprecipitation experiments.The membranes in the cell lysate were solubilized by the additionof 1% Triton X-100, and Pga1-6myc was precipitated using theanti-myc mAb from the cleared lysate. The GFP-tagged Gpi18 wasclearly detected in the precipitate fraction by immunoblotting(Figure 7D). Therefore, Gpi18 and Pga1 not only colocalizedin the ER but also had a physical interaction in vivo.

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Figure 7. Pga1 and Gpi18 proteins colocalized in the ER and were found in a complex in the Triton X-100–solubilized lysate. (A) The fluorescent image of GFP-Gpi18 and the indirect immunofluorescent staining image of Pga1-6myc were overlapping (merge). (B) Subcellular fractionation of GFP-Gpi18 was performed as described in Figure 2B. (C) Solubilization test of GFP-Gpi18 was performed as in Figure 2C. (D) The cleared lysate of the cells having either Pga1-6myc or untagged Pga1 in addition to GFP-Gpi18 was subjected to immunoprecipitation using anti-myc mAb, and GFP-Gpi18 and Pga1-6myc were detected by SDS-PAGE and Western blotting.

Pga1 is a Novel Subunit of Glycosylphosphatidylinositol-Mannosyltransferase II
Because the pga1-1 mutant cells showed defects in the modificationof the GPI anchor to the Gas1 precursor in the ER and otherpotential GPI-anchored proteins at 37°C, its temperature-sensitivegrowth defect was suppressed by the introduction of multicopyGPI18 gene, and Pga1 and Gpi18 were ER-membrane protein andfound in a complex in the Triton X-100-solubilized lysate, wesuspected that Pga1 and Gpi18 might cooperate in functioningas the enzyme to produce the GPI anchor. It was reported thatthe GPI18-depleted cell accumulated the GPI precursor "lipid004-1," which was identified as Man[EtN-P]-GlcN-PI (Fabre etal., 2005

); thus, we tested whether the pga1 mutant accumulatesthe same GPI precursor. For this purpose, we constructed theP_GAL1-GPI18 strain and gpi18^ts mutants. Screening for gpi18^tsmutants was performed by the same method by which the pga1^tsmutants were constructed. As a result, we obtained 7 gpi18^tsalleles and replaced the GPI18 gene on the chromosome of BY4741with gpi18-6 for the further analysis. To analyze for accumulationof GPI anchor precursors, the cells were metabolically labeledwith [³H]inositol, after which lipids were extracted from thecells and separated by TLC. [³H]Inositol-containing lipids onthe TLC were detected by autoradiography. As shown in Figure 8,the pga1^ts mutants and the gpi18^ts mutants accumulated a spotof the same RF at 37°C (Figure 8A, lanes 6 and 8, and B,lanes 6, 8, 10, and 12). This spot was also detected in thesample of the transcription arrested cells of the P_GAL1-GPI18promoter shut-off mutant in SD (Figure 8A, lane 4); so, thiscorresponds to the "lipid 004-1", namely, Man[EtN-P]-GlcN-PI.However, this spot was not detected in the wild type or ${Delta}$ gpi7at 25 or 37°C (Figure 8A, lanes 9 and 10, and B, lanes 1–4),and moderate accumulation was detected in the pga1^ts or thegpi18^ts mutant cells at 25°C (Figure 8A, lanes 5 and 7,and B, lanes 5, 7, 10, and 11). Therefore, the functional Pga1was necessary for the enzyme activity of GPI-MT II. We concludedthat Pga1 is an essential subunit of GPI-MT II. The accumulationof the lipid 004-1 in pga1-1 and gpi18-6 mutants was complementedby the introduction of the wild-type gene on CEN plasmid (Figure 8C).The presence of a small amount of the lipid 004-1 in pga1-1/PGA1may be caused by codominance of the pga1-1 mutation (Figure 8C,lane 4). On the contrary, the introduction of the high-copy-suppressorgenes on 2µ plasmid did not diminish the accumulation(Figure 8D).

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Figure 8. The temperature-sensitive pga1 mutants accumulated the same GPI anchor precursor that was accumulated in the Gpi18-deprived cells. (A) The myo-2-[³H]inositol-labeled lipids were extracted, developed on a TLC plate in CHCl₃/CH₃OH/H₂O (5:5:1, vol/vol), and detected by autoradiography. The wild-type (lanes 1 and 2) or P_GAL1-GPI18 (lanes 3 and 4) cells were grown at 30°C in SG (lanes 1 and 3) or SD (lanes 2 and 4). An intermediate lipid (lipid 004-1, indicated by the arrowhead) accumulated in the sample of lane 4 in which the expression of GPI18 was repressed for 20 h in the glucose-containing medium. The wild-type (lanes 9 and 10), pga1-1 (lanes 5 and 6), or gpi18-6 (lanes 7 and 8) ts mutant cells were labeled at either 25°C (lanes 5, 7, and 9) or 37°C (lanes 6, 8, and 10). An accumulation of the indicated GPI biosynthetic precursor was found in lanes 5, 6, 7, and 8. (B) The wild-type (WT, lanes 1 and 2), ${Delta}$ gpi7 (lanes 3 and 4), pga1-1 (lanes 5 and 6), pga1-3 (lanes 7 and 8), gpi18-3 (lanes 9 and 10), or gpi18-6 (lanes 11 and 12) cells were grown at either 25°C (lanes 1, 3, 5, 7, 9, and 11) or 37°C (lanes 2, 4, 6, 8, 10, and 12), and labeled with myo-2-[³H]inositol, and the accumulation of the GPI biosynthetic precursor was analyzed as in described in A. The intermediate lipid 004-1 is indicated by the arrowhead. (C) The complementation of the lipid 004-1 (arrowhead) accumulation in the pga1-1 (lanes 1–4) or gpi18-6 (lanes 5–8) cells by introducing PGA1 (lanes 3 and 4) or GPI18 (lanes 7 and 8) on CEN plasmid was examined. The mutants transformed with pRS316 were used as the controls (lanes 1, 2, 5, and 6). (D) The suppression of the lipid 004-1 (arrowhead) accumulation in pga1-1 (lanes 1–4) or gpi18-6 (lanes 5–8) cells by introducing GPI18 (lanes 3 and 4) or PGA1 (lanes 7 and 8) on 2µ plasmid was examined. The mutants transformed with pRS426 were used as the controls (lanes 1, 2, 5, and 6).

Gpi18 Is Stable Irrespective of Pga1
GPI-MT I also consists of two proteins in mammalian cells, PIG-Mand PIG-X (Ashida et al., 2005

). PIG-M is a multimembrane-spanningprotein like Gpi18, and PIG-X is a protein with a single transmembranedomain like Pga1. Because PIG-X was reported to stabilize PIG-M,we speculated that the loss of Pga1 or 37°C incubation ofts allele of Pga1 would cause the destabilization of Gpi18.To test this possibility, GFP-Gpi18 was expressed in P_GAL1-PGA1mutant or pga1-1 mutant cells. Even after P_GAL1-PGA1 was incubatedin SD medium for 20 h when the lipid 004-1 significantly accumulated(data not shown), no reduction in the amount of GFP-Gpi18 wasobserved (Figure 9A). Similarly, incubation at 37°C for2 h did not affect the stability of GFP-Gpi18 in pga1^ts mutants(Figure 9B), although the 105-kDa proGas1 was significantlyaccumulated (data not shown). Therefore, the stability of Gpi18is independent of Pga1.

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Figure 9. The stability of Gpi18 was not affected in pga1 mutants. (A) GFP-Gpi18 was expressed in the WT (lanes 1 and 4) or P_GAL1-PGA1 (KSY308, lanes 2 and 5; KSY309, lanes 3 and 6) cells. After 20-h incubation in SG (lanes 1–3) or SD medium (lanes 4–6), GFP-Gpi18 was detected by SDS-PAGE and Western blotting. KSY308 and KSY309 are independent isolates of the same construction. (B) GFP-Gpi18 was expressed in the WT (lanes 1 and 2) or in the pga1^ts mutants (pga1-1, lanes 3 and 4; pga1-2, lanes 5 and 6). After 2-h incubation at 25°C (lanes 1, 3, and 5) or at 37°C (lanes 2, 4, and 6), GFP-Gpi18 was detected as described in A.

Human PIG-V Rescues the Viability of ${Delta}$ pga1 Cells
It is curious that PGA1 has homologues only in fungi but notin higher eukaryotes including mammals, because all S. cerevisiaegenes identified so far to be involved in GPI synthesis or anchoringhave their mammalian homologues. So, it is natural to assumethe existence of a counterpart of Pga1 in mammalian cells. Ifthe Pga1 counterpart exists, two probable reasons why thereis no apparent PGA1 homologue were concerned. The first is thatthe sequence similarity between the two proteins is not highenough to be detected by homology search, although they arefunctionally homologous. The other is that the function of mammalianPIG-V contains not only that of Gpi18 but also that of Pga1.To discern which possibility is likely, we introduced the FLAG-humanPIG-V on pRS316 (pFLAG-hPIG-V, a generous gift from Dr. TarohKinoshita, Research Institute for Microbial Disease; Osaka;Kang et al., 2005

) to the heterozygous PGA1/ ${Delta}$ pga1::kanMX4 diploidcells. The spores of the transformants were dissected to assessthe complementation by tetrad analysis. As shown in Figure 10A,most tetrads from PGA1/ ${Delta}$ pga1::kanNMX4 diploid cells harboringpFLAG-hPIG-V generated four viable haploid progenies with twoof normal growth and two of slow growth. The slow growth cellswere ${Delta}$ pga1 alleles whose viability was dependent on the pFLAG-hPIG-Vbecause they were resistant to Geneticin (G418; Invitrogen)and lethal on 5-FOA plate, and the normal growth cells werewild-type cells because they were sensitive to G418 and grewnormally on the 5-FOA plate. The same result was obtained whenthe pFLAG-hPIG-V was introduced to the GPI18/ ${Delta}$ gpi18::kanMX4 diploid;two normal growth haploids sensitive to G418 and two slow growthhaploids resistant to G418 were observed in most tetrads (Figure 10B).These results indicate that human PIG-V rescues the viabilityof not only ${Delta}$ gpi18 but also ${Delta}$ pga1. Furthermore, the introductionof GPI18 to ${Delta}$ pga1 even on 2µ plasmid could not rescue theviability, indicating that the function of Gpi18 is completelydistinct from that of Pga1. Thus, human PIG-V is strongly suggestedto possess the functions of both Gpi18 and Pga1 of S. cerevisiae.

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Figure 10. Human PIG-V rescues the viability of both ${Delta}$ gpi18 and ${Delta}$ pga1. (A) The heterozygous PGA1/ ${Delta}$ pga1:: kanMX4 diploid cells were transformed with pFLAG-hPIG-V and were sporulated. The spores were dissected to assess the complementation by tetrad analysis. The genotypes of the numbered progenies (1–8) were checked by streaking the indicated cells on the G418 plate and the 5-FOA plate. (B) The heterozygous GPI18/ ${Delta}$ gpi18::kanMX4 diploid cells were transformed with pFLAG-hPIG-V and were sporulated. The genotypes of the numbered progenies (9–16) were checked as described in A.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Enormous efforts have been made to identify the genes requiredfor the yeast GPI biosynthesis. Two major strategies were generallytaken in S. cerevisiae by most researchers; one was to screenthe mutants defective in inositol incorporation, and the otherwas to find homologues with mammalian proteins that are provento be involved in GPI biosynthesis. Despite these intensivestudies, a flippase to move the GPI intermediate across themembrane and a GPI remodelase to introduce a ceramide to GPIthat already attached to the target proteins have not been identifiedso far. In contrast, because an in vitro reaction of GPI synthesisusing purified enzymes and substrates has not been demonstratedyet, it is not possible to exclude an undiscovered participantin any step of GPI biosynthesis.

We focused on the characterization of the ER-localized essentialproteins whose functions remain unknown even after the enormouscomprehensive studies of S. cerevisiae. Our strategy uses theconstruction of temperature-sensitive mutants suitable for bothphenotypic and genetic studies. The temperature-sensitive pga1mutants showed defects in the processing and transport of theGPI-anchored Gas1 protein (Figure 3A) and biochemical analysisindicated that GPI anchor synthesis was defective (Figure 4).Genetic analysis identified the GPI18 gene as a multicopy suppressorof the growth defect of pga1-1 (Figure 6A). Gpi18 was reportedto be GPI-MT II, which adds Man to Man-GlcN-PI, and the mutantsin pga1 as well as gpi18 accumulated the same intermediate,Man[EtN-P]-GlcN-PI (Figure 8). Gpi18 and Pga1 not only colocalizedin the ER membrane but also were found in a complex after TritonX-100 solubilization of the cell lysate (Figure 7). From allthese results, we concluded that Pga1 is a novel subunit ofGPI-MT II that collaborates with another subunit Gpi18 (Figure 10).

As shown in Figure 11, several steps in GPI biosynthesis arereported to be carried out by the participation of multipleproteins (Kinoshita and Inoue, 2000; Pittet and Conzelmann,2006). Both mammalian and budding yeast GPI-MT I are a complexof a multimembrane-spanning protein (PIG-M/Gpi14) and a singlemembrane-spanning protein (PIG-X/Pbn1). Most GPI-MT polypeptideshave a DXD motif, which is generally required for the activityof glycosyltransferase. Because PIG-M and Gpi14 have a DXD sequence,the multimembrane-spanning subunit probably represents the catalyticsubunit. The molecular function of PIG-X and Pbn1 is unknown,but PIG-X was reported to be required for stability of PIG-M(Ashida et al., 2005). So, the single membrane-spanning subunitmay play a structural role for the partner. However, as forPga1, neither repression of PGA1 by the GAL1 promoter shut-offnor incubation of the pga1-1 mutant at 37°C affected theamount of Gpi18 (Figure 9), suggesting that Pga1 is not requiredfor the stability of its partner. The overexpression of GPI18could not rescue the lethality of ${Delta}$ pga1. It only rescued thetemperature sensitivity of pga1^ts. Conversely, PGA1 overexpressionsuppressed the temperature sensitivity of gpi18^ts (Figure 6A).We immunoprecipitated Pga1-6myc from the digitonin-solubilizedmembrane fraction with the anti-myc antibody, but we could notdetect any other interacting protein except Gpi18 in the coprecipitatedproteins (data not shown). These data indicate that both Pga1and Gpi18 would be required to generate the overall structurenecessary for the substrate recognition and enzymatic activityof yeast GPI-MT II.

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Figure 11. The mannosylation process in GPI anchor synthesis. Pga1 is a partner of Gpi18. GPI-MT I and GPI-MT II are composed of protein complex. The GPI-MT subunits containing a DXD motif are shown in bold.

The sequences of polypeptides of GPI-MT II do not contain aDXD motif, which is commonly present in glycosyltransferases.Instead, Gpi18 and PIG-V has a structural feature common withPmt2-family proteins (Kang et al., 2005

). The Pmt2-family proteinsare O-mannosyltransferases, which have multiple transmembranedomains but no DXD motif. They have two conserved hydrophilicloops that face the ER lumen. One loop is between the firstand second transmembrane domains and the other is between thefifth and sixth. The first loop of each Pmt2-family proteinhas a Trp-Asp motif as well as Gpi18 and PIG-V. In CHO PIG-Vmutants, single amino-acid substitutions of W66L or D67A inthe conserved Trp-Asp motif were responsible for the mutantphenotype (Kang et al., 2005

). Considering this result and structuralfeatures, Gpi18 is likely to be a catalytic subunit of the yeastGPI-MT II, but it requires the partner Pga1 for the activity.

No obvious Pga1 homologue was found in mammalian cells. Thereare several possible explanations why Pga1 is required onlyin fungi. First, the Pga1 function is necessary only in yeastcells and completely specific to yeast. Second, there is a functionalhomologue with very low similarity. Third, PIG-V possesses thefunctions of both Gpi18 and Pga1. We supposed that the firstpossibility was unlikely because the GPI biosynthetic pathwayis conserved between the yeast and the mammalian cell very wellso intermediates and enzymes in the pathway should be common.The second possibility seemed likely; however, the third possibilitywas most likely because the expression of the human PIG-V genein both ${Delta}$ gpi18 and ${Delta}$ pga1 cells could suppress their lethality(Figure 10). So, it is natural to suppose that the two yeastproteins compose the GPI-MT II complex, which is functionallyhomologous to the single human PIG-V protein. Compared withhuman PIG-V, the hydrophilic segments at the both sides of theseventh transmembrane domain are missing in yeast Gpi18 (Figure 4of Kang et al., 2005). It is possible that Pga1 compensatesfor the function of these missing segments by forming a complexwith Gpi18 in the membrane. Because the PIG-V homologue in fruitfly has similar missing stretches, it may require a homologueof Pga1 for its activity.

Considering that both GPI-MT I and GPI-MT II are composed of(at least) two subunits in S. cerevisiae, it is natural to askwhether GPI-MT III or IV forms a similar complex, because theyare using substrates with structures similar to those used byGPI-MT I and GPI-MT II. The proteins that have been proved tobe responsible for the mannosylation in GPI-MT III and IV untilnow are Gpi10 and Smp3, respectively, both of which are multimembrane-spanningproteins like Gpi14 and Gpi18. It would be very interestingto perform the multicopy suppressor screening of gpi10 or smp3temperature-sensitive mutants to see whether there would beany partner proteins to them.

ACKNOWLEDGMENTS

We thank Drs. S. Kagiwada and M. Tokunaga for kindly providingantisera; Dr. Taroh Kinoshita for kindly providing the humanPIG-V expression plasmids; Chihiro Akimoto and Atsushi Kamiyafor help in preliminary characterization of PGA1; Mariko Umemuraand Dr. Takehiko Yoko-o for valuable advices in the analysisof GPI precursors; Dr. Hironori Inadome, Dr. Shah Alam Bhuiyanand Dr. Hiroyuki Adachi for helpful discussions. This work wassupported by a Research Fellowship for Young Scientists fromthe Japan Society for the Promotion of Science (to K.S.), grants-in-aidfor Scientific Research from the Japan Society for the Promotionof Science (to Y.N.), and grants for "Bioarchitect Research"from the Institute of Physical and Chemical Research (RIKEN)of Japan (to K.Y.) and a grant from the Noda Institute of ScientificResearch (to K.Y.).

Footnotes

This was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E07-03-0258)on July 5, 2007.

Address correspondence to: Koji Yoda (asdfg{at}mail.ecc.u-tokyo.ac.jp).

Abbreviations used: ALP, alkaline phosphatase; CPY, carboxypeptidase Y; endoH, endoglycosidase H; ER, endoplasmic reticulum; EtN-P, phosphoethanolamine; GFP, green fluorescent protein; GlcN, glucosamine; GPI, glycosylphosphatidylinositol; GPI-MT, GPI-mannosyltransferase; Man, mannose; PI, phosphatidylinositol; SGD, Saccharomyces Genome Database.

REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Ashida, H., Hong, Y., Murakami, Y., Shishioh, N., Sugimoto, N., Kim, Y. U., Maeda, Y., and Kinoshita, T. (2005). Mammalian PIG-X and yeast Pbn1p are the essential components of glycosylphosphatidylinositol-mannosyltransferase I. Mol. Biol. Cell 16, 1439–1448.[Abstract/Free Full Text]

Ballou, C. E. (1990). Isolation, characterization, and properties of Saccharomyces cerevisiae mnn mutants with nonconditional protein glycosylation defects. Methods Enzymol 185, 440–470.[Medline]

Belden, W. J., and Barlowe, C. (2001). Deletion of yeast p24 genes activates the unfolded protein response. Mol. Biol. Cell 12, 957–969.[Abstract/Free Full Text]

Davierwala, A. P. et al. (2005). The synthetic genetic interaction spectrum of essential genes. Nat. Genet 37, 1147–1152.[CrossRef][Medline]

Davydenko, S. G., Feng, D., Jäntti, J., and Keränen, S. (2005). Characterization of GPI14/YJR013w mutation that induces cell wall integrity signaling pathway and results in increased protein production in Saccharomyces cerevisiae. Yeast 22, 993–1009.[CrossRef][Medline]

Doering, T. L., and Schekman, R. (1996). GPI anchor attachment is required for Gas1p transport from the endoplasmic reticulum in COP II vesicles. EMBO J 15, 182–191.[Medline]

Duenas, E., Revuelta, J. L., del Rey, F., and Vazquez de Aldana, C. R. (1999). Disruption and basic phenotypic analysis of six novel genes from th