Two Endoplasmic Reticulum () Membrane Proteins That Facilitate ER-to-Golgi Transport of Glycosylphosphatidylinositol-anchored Proteins

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Vol. 10, Issue 4, 1043-1059, April 1999

Two Endoplasmic Reticulum (ER) Membrane Proteins That Facilitate ER-to-Golgi Transport of Glycosylphosphatidylinositol-anchored Proteins

Wolfgang P. Barz,^* and Peter Walter

^*Department of Membrane Biochemistry, Max-Planck-Institute for Biochemistry, 82152 Martinsried, Germany; and Howard Hughes Medical Institute and Department of Biochemistry and Biophysics, University of California Medical School, San Francisco, California 94143-0448

Submitted October 23, 1998; Accepted January 29, 1999
Monitoring Editor: Randy W. Schekman

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Many eukaryotic cell surface proteins are anchored in the lipid bilayer through glycosylphosphatidylinositol (GPI). GPI anchorsare covalently attached in the endoplasmic reticulum (ER). Themodified proteins are then transported through the secretory pathwayto the cell surface. We have identified two genes in Saccharomycescerevisiae, LAG1 and a novel gene termed DGT1 (for "delayed GPI-anchoredprotein transport"), encoding structurally related proteins withmultiple membrane-spanning domains. Both proteins are localizedto the ER, as demonstrated by immunofluorescence microscopy. Deletionof either gene caused no detectable phenotype, whereas lag1 $Delta$ dgt1 $Delta$ cells displayed growth defects and a significant delay in ER-to-Golgitransport of GPI-anchored proteins, suggesting that LAG1 and DGT1encode functionally redundant or overlapping proteins. The rateof GPI anchor attachment was not affected, nor was the transportrate of several non-GPI-anchored proteins. Consistent with a roleof Lag1p and Dgt1p in GPI-anchored protein transport, lag1 $Delta$ dgt1 $Delta$ cells deposit abnormal, multilayered cell walls. Both proteinshave significant sequence similarity to TRAM, a mammalian membraneprotein thought to be involved in protein translocation acrossthe ER membrane. In vivo translocation studies, however, did notdetect any defects in protein translocation in lag1 $Delta$ dgt1 $Delta$ cells,suggesting that neither yeast gene plays a role in this process.Instead, we propose that Lag1p and Dgt1p facilitate efficientER-to-Golgi transport of GPI-anchoredproteins.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

A large number of proteins are transported across or integrated into the endoplasmic reticulum (ER)¹ membrane (for review, see Walter and Johnson, 1994; Rapoportet al., 1996). These include most integral membrane and secretedproteins and most proteins destined to be stored in the lumenof intracellular organelles such as the ER, Golgi apparatus, lysosomes,and endosomes. In yeast, translocation of secretory precursorsmay follow one of two pathways (Ng et al., 1996). Membrane transitmay occur either cotranslationally, in a reaction that requirestargeting of ribosomes to the ER membrane, or posttranslationally,in an alternate pathway that allows polypeptides to traverse theER membrane after their synthesis has beencompleted.

Cotranslational translocation across the ER membrane is initiated by the binding of the signal recognition particle (SRP)to ribosomes synthesizing polypeptides with hydrophobic signalsequences (for review, see Walter and Johnson, 1994). Interactionof SRP with the SRP receptor, a heterodimeric protein on the cytosolicsurface of the ER membrane, targets the ribosome-nascent polypeptidecomplex to the ER membrane where a membrane complex termed the"translocon" catalyzes the transmembrane translocation of thenascent polypeptide. The core of the mammalian translocon consistsof the heterotrimeric Sec61p complex, which is essential for translocationof all proteins and forms a hydrophilic, protein-conducting channelspanning the entire membrane (Simon and Blobel, 1991; Crowleyet al., 1994).

Another component of the mammalian translocon is the multispanning membrane protein termed "trans-locating chain-associatedmembrane protein" (TRAM) which was found to be a principal cross-linkingpartner of different secretory proteins that are in transit acrossthe membrane (Görlich et al., 1992). TRAM becomes cross-linkedmostly to the charged, N-terminal region of the signal sequence(Görlich et al., 1992) and is no longer cross-linked to the nascentchain once the signal sequence is cleaved off by the signal peptidase(Mothes et al., 1994). Furthermore, nascent chains that carrya nonfunctional signal sequence are not cross-linked to TRAM,suggesting that nascent chains contact TRAM during an early phaseof the translocation process (Jungnickel and Rapoport, 1995).

Protein translocation across the ER membrane can be reproduced using proteoliposomes reconstituted from detergent-solubilizedER membrane proteins (for review, see Rapoport et al., 1996).Interestingly, the heterotrimeric Sec61p complex, together withthe SRP receptor, is sufficient for the translocation of somepolypeptides into reconstituted proteoliposomes (Görlich andRapoport, 1993). However, the translocation of most polypeptidesdepends on the presence of TRAM (Voigt et al., 1996). Whethera protein requires TRAM for translocation is determined by structuralfeatures of its signal sequence, supporting the notion that TRAMfunctions at an early phase of the translocation process (Voigtet al., 1996). Furthermore, TRAM was recently shown to be involvedin regulating "translocational pausing," a mechanism by whichcertain nascent secretory proteins are transiently exposed tothe cytosol (Hegde et al., 1998). That study suggested that onerole of TRAM may be to prevent cytosolic exposure of already translocateddomains of the nascent chain. In contrast, studies on the integrationof an integral membrane protein revealed cross-links between TRAMand the transmembrane segment rather late in the integration process,when the transmembrane domain can no longer be cross-linked toSec61p and has laterally left the core of the translocon (Do etal., 1996). However, a functional role for TRAM in the releaseof transmembrane sequences into a lipid environment has not yetbeen demonstrated. Thus, the precise role of the mammalian TRAMprotein remainsobscure.

After translocation into the ER lumen, many proteins are further modified by posttranslational modifications such as signalsequence cleavage, side chain glycosylation, and disulfide bondformation. One additional modification is the addition of a glycosylphosphatidylinositol(GPI) anchor to the C terminus of the protein (for review, seeTakeda and Kinoshita, 1995). GPI-anchored proteins represent asubclass of cell surface proteins serving diverse cellular functionssuch as transmembrane signaling, cell wall synthesis, and celladhesion (Englund, 1993; Klis, 1994). In yeast, GPI-anchoringis an essential process for viability (Leidich et al., 1994; Hamburgeret al., 1995; Schönbächler et al., 1995; Vossen et al., 1995).

GPI proteins are synthesized as precursors with two signal sequences: a classical cleavable signal sequence at the N terminusrequired for translocation of the protein into the ER lumen, andan additional hydrophobic region at the C terminus of the protein,which directs GPI anchoring in the lumen of the ER. During orafter translocation of the protein into the ER, the C-terminalhydrophobic region is removed and replaced en bloc with a complete,preformed GPI anchor, which has been synthesized by the stepwiseaddition of sugars and phosphoethanolamine to phosphatidylinositol(Englund, 1993). Several of the genes involved in the synthesisof the yeast GPI anchor have been cloned and characterized (Hamburgeret al., 1995; Leidich et al., 1995; Schönbächler et al., 1995;Benghezal et al., 1996).

GPI anchors have been proposed to play a role in protein sorting (Takeda and Kinoshita, 1995). In yeast, GPI anchor attachmentis necessary for exit of GPI proteins from the ER (Nuoffer etal., 1993; Doering and Schekman, 1996). Only after anchor attachmentare GPI proteins packaged into transport vesicles that leave theER and are transported to the Golgi compartment (Schekman andOrci, 1996). How specific cargo proteins are recruited and concentratedinto ER-derived transport vesicles is still poorly understoodand the subject of intense investigation; GPI-anchored proteinsmay have unique requirements for this process (Brown, 1992; Brownand Rose, 1992; Futerman, 1995).

In this paper, we present evidence for two proteins that facilitate the vesicular transport of GPI proteins. In an attemptto identify the molecular function of TRAM, we identified twoyeast proteins with significant sequence similarity to TRAM thatare localized to the ER membrane. Unexpectedly, we found no evidencethat these membrane proteins are involved in protein translocationacross the ER membrane; instead, they appear to be specificallyinvolved in the ER-to-Golgi transport of GPI-anchoredproteins.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Yeast Strains, Media, Reagents, and General Methods

Saccharomyces cerevisiae strains used in this study are listed in Table 1. Complete medium (YPD) and synthetic minimal mediawith glucose or galactose as the carbon source were used as described(Sherman, 1991). Synthetic complete minimal medium lacking inositol(SC $-$ inositol) was prepared as published before (Culbertson andHenry, 1975). Growth rates were determined quantitatively at 15,22, 30, 37, 39, and 40°C by measuring the optical density at 600nm (OD₆₀₀) of aliquots taken from exponentially growing YPD liquidcultures.

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Table 1. Haploid yeast strains used in this study

Recombinant DNA techniques were performed using standard techniques (Sambrook et al., 1989). Yeast strains were transformedwith plasmids using electroporation (Becker and Guarente, 1991)or lithium acetate procedures (Ito et al., 1983). Western blotswere visualized using enhanced chemiluminescence (Amersham, ArlingtonHeights, IL) as described by the manufacturer. SDS-PAGE was performedon 10-15% gradient gels. Chemicals were from Sigma Chemicals (St.Louis, MO) unless otherwise noted. DNA sequencing was performedusing an Applied Biosystems A220 fluorescent DNA sequencer (PerkinElmer-Cetus, Foster City, CA) and cyclesequencing.

Disruption of LAG1 and DGT1

The chromosomal deletion alleles lag1 $Delta$ ::HIS3 and dgt1 $Delta$ ::ADE2 were created by replacing the entire coding sequences of LAG1and DGT1 with yeast-integrative plasmids (Sikorski and Hieter,1989). To disrupt LAG1, the noncoding flanking regions of thisgene (400-600 base pairs [bp]) were amplified by genomic PCR usingoligonucleotides that incorporated EcoRI restriction sites atthe ends of the fragments distant from LAG1 and EcoRV and XbaIsites at the inside ends. These fragments were then digested withthe relevant restriction enzymes and cloned in a three-way ligationinto EcoRV- and XbaI-cut pRS303 (HIS3; Sikorski and Hieter, 1989).The resulting plasmid, pWB281, was linearized with EcoRI and usedto transform haploid W303-1B cells to His⁺ prototrophy. One of the His⁺ transformants was purified and designated WBY283. Correct chromosomaldeletion of LAG1 was confirmed by extensive genomic PCR analysisusing several primer pairs specific for either the wild-type alleleLAG1 or the disruption allele lag1 $Delta$ ::HIS3.

A similar strategy was used to replace the entire coding region of DGT1 with a yeast-integrative vector, pSO403 (ADE2; kindlyprovided by S.C. Ogg, Department of Biochemistry, University ofDundee, Dundee, United Kingdom). pSO403 had been constructed bysubcloning a 2.3-kilobase (kb) BglII-BglII fragment containingthe ADE2 gene from S. cerevisiae (Stotz and Linder, 1990) intothe BamHI site of pBluescript II SK(+) (Stratagene, La Jolla,CA). The 5'- and 3'-flanking sequences of DGT1 (400-600 bp) wereamplified by genomic PCR and cloned in a three-piece ligationinto PstI- and XhoI-digested pSO403. The resulting plasmid, pWB280,was linearized with EcoRI and used to transform haploid W303-1Acells to Ade⁺ prototrophy. Correct replacement of DGT1 was confirmed in oneAde⁺ transformant (termed WBY286) by genomic PCRanalysis.

Diploid W303 cells were also transformed with EcoRI-linearized pWB280, giving rise to a heterozygous chromosomal disruptionof DGT1. Diploid Ade⁺ transformants were induced to sporulate in liquid sporulationmedia, and asci were dissected into tetrads. Both at 25 and 37°C,all tetrads analyzed gave rise to four equally well-growing colonies,showing that DGT1 is not important forgrowth.

Generation of a lag1 $Delta$ dgt1 $Delta$ Double Disruption Mutant

WBY283 and WBY286 were mated to construct a diploid that is heterozygous for both LAG1 and DGT1. The resulting His⁺Ade⁺ diploid (designated WBY600) was sporulated in liquid sporulationmedium, and asci were dissected into tetrads. All tetrads gaverise to four viable spores, most of which grew with the wild-typerate, whereas some grew with a drastically reduced rate. Markersanalysis revealed that the growth defect always cosegregated withthe His⁺Ade⁺ phenotype. Genomic PCR analysis of all four colonies producedfrom spores of a single tetrad of nonparental ditype confirmedthat the slowly growing His⁺Ade⁺ colonies contain the lag1 $Delta$ ::HIS3 and dgt1 $Delta$ ::ADE2 disruptionsbut not the LAG1 and DGT1 wild-type alleles. One haploid lag1 $Delta$ ::HIS3dgt1 $Delta$ ::ADE2 clone was designatedWBY616.

Cloning and Epitope Tagging of LAG1 and DGT1

LAG1 and DGT1 were amplified with flanking sequences (350-550 bp) by genomic PCR using Vent polymerase (New England Biolabs,Beverly, MA) and oligonucleotides that incorporated restrictionsites at their 5' ends (HindIII and XbaI for the amplificationof LAG1; SacII and XhoI for amplifying DGT1). The resulting 2.0-to 2.2-kb DNA fragments were digested with the relevant restrictionenzymes and cloned into the centromeric vector pRS316 (URA3; Sikorskiand Hieter, 1989) digested with the same enzymes. Sequence analysisrevealed that the inserts of the resulting plasmids, pWB98 (carryingLAG1) and pWB95 (carrying DGT1), agreed with the published genomicsequence. pWB96 was constructed by inserting the 2.0-kb SacII-XhoIfragment of pWB95 (bearing DGT1) into the centromeric vector pRS314(TRP1; Sikorski and Hieter, 1989) to replace the SacII-XhoI fragmentin thepolylinker.

To construct an epitope-tagged HA-Dgt1p protein, a double-stranded DNA cassette was assembled by annealing the complementaryoligonucleotides 5'-TCGACATACCCATATGATGTTCCAGATTACGCT-3' and 5'-TCGAAGCGTAATCTGGAACATCAT-ATGGGTATG-3'.The protruding termini of this cassette are identical to thosegenerated by the restriction endonuclease SalI. One copy of thisconstruct was ligated into SalI-digested pWB96. The resultingplasmid, pWB94, carries an N-terminal hemagglutinin (HA) epitopeinserted between the first and second amino acids of Dgt1p. Bothstrands of the modified region of pWB94 were sequenced to showthat only the desired mutation had beenintroduced.

Haploid yeast strains carrying pWB94, pWB95, pWB96, or pWB98 were constructed by individually transforming these plasmidsinto the heterozygous diploid WBY600 (see above). Trp⁺ or Ura⁺ transformants were sporulated in liquid sporulation medium. Asciwere dissected into tetrads and allowed to germinate on minimalplates lacking tryptophan or uracil. All Ade⁺ His⁺ spores (containing the disruption alleles lag1 $Delta$ ::HIS3 and dgt1 $Delta$ ::ADE2)that were also Trp⁺ (containing pWB94 or pWB96) or Ura⁺ (containing pWB95 or pWB98) gave rise to colonies of identicalsize as the Ade His colonies (containing the wild-type alleles). The resulting haploidswere purified and termed WBY739, WBY741, WBY743, and WBY777 (seeTable 1).

Antibodies

Monoclonal anti-HA ascites fluid was purchased from Babco (Berkeley Antibody, Richmond, CA). TRITC-conjugated donkey anti-mouseimmunoglobulin G (IgG) and donkey anti-rabbit IgG were purchasedfrom Jackson ImmunoResearch (West Grove, PA). Polyclonal anti-Kar2pantibodies were prepared in our laboratory using Kar2p overexpressedin Escherichia coli from a clone kindly provided by M. Rose (PrincetonUniversity, Princeton, NJ). The following polyclonal antiserawere kindly provided by the indicated investigators: anti-CPY,R. Schekman (University of California, Berkeley, CA); anti-DPAPB, T. Stevens (University of Oregon, Eugene, OR); anti-Gas1p,A. Conzelmann (Université de Fribourg, Fribourg, Switzerland);and anti-Yap3p, Y. Bourbonnais (Université Laval, Québec,Canada).

Immunofluorescence

The intracellular location of HA-Dgt1p was examined by indirect immunofluorescence performed essentially as described (Pringleet al., 1991). Strains expressing HA-Dgt1p (WBY739) or untaggedDgt1p (WBY743) were grown at 30°C to early exponential growthphase (10⁶-10⁷ cells/ml) in SC medium lacking tryptophan. Cells were fixed for2 h with 3.7% formaldehyde in the medium. Antibody incubationswere performed in a humid chamber at 25°C for 1 h. HA-Dgt1p wasdetected using a 1:5000 dilution of monoclonal anti-HA serum.Polyclonal antibodies against Kar2p were used at a dilution of1:10,000. Bound primary antibodies were decorated with TRITC-conjugateddonkey anti-mouse IgG or donkey anti-rabbit IgG diluted 1:200.Slides were mounted in 90% glycerol containing 1 mg/ml p-phenylenediamine,pH 9.0, and 1 µg/ml DAPI. Cell remnants were examined at 1000-foldmagnification on a Zeiss Axioskop microscope (Carl Zeiss, Thornwood,NY). Images were recorded on Eastman Kodak (Rochester, NY) TMAX400 film with a Zeiss MC 80 camera andcontroller.

Electron Microscopy

Yeast cells were grown to early logarithmic phase at 30°C in YPD medium and prepared for electron microscopy by fixation withglutaraldehyde and KMnO₄ (Kaiser and Schekman, 1990). Fixed cellswere dehydrated through a graded ethanol series and embedded inSpurr's resin (PolyScience, Niles, IL) overnight at 60°C. Thinsections (thickness, 50-60 nm) were stained with uranyl acetateand lead citrate and examined with a Zeiss 10 CA electronmicroscope.

In Vivo Labeling with ³⁵S and Immunoprecipitations

Yeast cells were grown to early logarithmic phase in YPD medium at 30°C except for sec13-1 cells, which were grown at 22°Cand shifted to 37°C for 90 min before labeling. Cells were harvestedand washed three times with SC minimal medium lacking methionine.For in vivo translocation studies, pulse labeling with [³⁵S]methionine and [³⁵S]cysteine (ProMix ³⁵S cell labeling mix; Amersham) and non-native immunoprecipitationswere performed as described before (Hann and Walter, 1991). Pulse-chaseexperiments were performed by pulse labeling cells for 2 min at30°C with 50 µCi/OD₆₀₀ ProMix followed by the addition of a 1/50vol of 200 mM methionine/200 mM cysteine (10,000-fold molar excess).During the 30-min chase period, aliquots containing 5 OD₆₀₀ unitswere collected at the indicated times. Cell lysis and immunoprecipitationswere performed as described (Hann and Walter, 1991). The immunoprecipitateswere analyzed by SDS-PAGE on 10-15% gradient gels, followed byexposure and quantitation of the gel on a PhosphorImager (MolecularDynamics, Sunnyvale,CA).

GPI Anchor Attachment Assay

Yeast cells were grown at 22°C to early logarithmic phase in SC minimal medium. Twenty OD₆₀₀ units were collected, washedthree times with SC $-$ inositol, resuspended in 1.0 ml of SC $-$ inositol, and preincubated for 5 min at 30°C (W303-1A and WBY616)or 37°C (RH2856). After the addition of 200 µCi of [³H]myo-inositol (Amersham), cells were incubated at 30°C (W303-1Aand WBY616) or 37°C (RH2856). At the indicated times, 400-µl aliquotswere removed and frozen in liquid nitrogen. NaN₃ and NaF wereadded to a 10 mM final concentration. The cells were thawed onice, washed twice in 10 mM NaN₃ and 10 mM NaF, resuspended in1 ml of a mixture of CHCl₃:CH₃OH:H₂O (10:10:3), and lysed by vortexingwith glass beads. The beads were removed, and proteins were precipitatedat 10,000 × g for 5 min and delipidated by reextracting the pellettwice with CHCl₃:CH₃OH:H₂O (10:10:3). The pellet was dried, resuspendedin protein sample buffer, and boiled for 5 min. After centrifugationat 10,000 × g for 5 min, the proteins were separated by SDS-PAGEand prepared for fluorography by soaking the gel for 10 min inAmplify(Amersham).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Characterization of Two Proteins in S. cerevisiae That Are Structurally Related to TRAM

To identify yeast homologues of TRAM, the genomic DNA sequence of S. cerevisiae was analyzed. A database search revealed twoyeast genes encoding proteins with significant sequence similarityto the mammalian TRAM protein (Figure 1): the previously describedgene LAG1, identified as a regulator of longevity and aging (D'melloet al., 1994; see DISCUSSION), and a novel ORF on chromosome XI(YKL008c). For reasons discussed below, we refer to this secondgene as DGT1, for "delayed GPI-anchored protein transport." Byconvention, the corresponding gene products are termed Lag1p andDgt1p, respectively. Both proteins have a predicted molecularmass of 48-49 kDa and show 70% sequence identity, suggesting thatthey may have similar or functionally redundant activities.

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Figure 1. Multiple alignment of the predicted amino acid sequence of TRAM homologues. The alignment includes the deduced protein sequence of S. cerevisiae LAG1 (D'mello et al. 1994

), S. cerevisiae YKL008c (termed DGT1 in this work), human TRAM (Görlich et al. 1992

), a human TRAM homologue (KIAA0057; Nomura et al. 1994

), and human UOG-1. The alignment was generated using the PileUp (Genetics Computer Group, Madison, WI) and BOXSHADE (Institute for Animal Health, Surrey, United Kingdom) programs. Gaps that were inserted during the alignment are denoted by dots. Potential membrane-spanning domains were predicted using four different algorithms: PepPlot (Kyte and Doolittle, 1982

), TMAP (Persson and Argos, 1994

), TMpred (Hofmann and Stoffel, 1993

), and TopPred2 (von Heijne, 1992

). The positions of these putative transmembrane domains are indicated by black bars above the alignment. N-linked glycosylation consensus sequences are underlined. Black boxes indicate identical residues, whereas gray boxes show amino acid similarity.

In addition to their homology to TRAM, the yeast proteins Lag1p and Dgt1p have a sequence similarity to two additional mammalianproteins (Figure 1). KIAA0057 is very closely related to TRAM(53% sequence identity; Nomura et al., 1994), whereas UOG-1 isa human ORF with less sequence similarity to TRAM (Lee, 1991).Over their entire lengths, both predicted proteins are 19-21%identical to Lag1p and Dgt1p. The functions of KIAA0057 and UOG-1are unknown. From sequence analysis, all family members are integralmembrane proteins, Lag1p, Dgt1p, TRAM, and KIAA0057 having sevenclusters of hydrophobic residues that are predicted to form membrane-spanningdomains (Figure 1, overlined), whereas UOG-1 is shorter and hasonly six predicted transmembraneregions.

Like many proteins with multiple membrane-spanning domains, all TRAM family members shown in Figure 1 do not contain N-terminalcleaved signal sequences. Lag1p and Dgt1p as well as TRAM andKIAA0057 have several potential N-linked glycosylation sites (Figure1, underlined). One remarkable feature of the two yeast proteinsis the presence of a stretch of acidic and hydroxylated aminoacids at the very C terminus (>75% Asp, Glu, Ser, or Thr overa range of 20-25 residues). The significance of this structuralfeature isunknown.

The C termini of all TRAM family members contain dilysine motifs (KKXX or KXKXX) known to be required for membrane proteinretrieval from the Golgi compartment back to the ER (Jackson etal., 1990). Therefore, these proteins are likely to be localizedto the ER or to shuttle between the ER and the Golgi apparatus.Because the ER retrieval signal has been shown to interact withcytosolic coatomer (COP) subunits (Cosson and Letourneur, 1994),the C termini of Lag1p and Dgt1p are likely to face thecytosol.

Cellular Localization of Dgt1p in the ER

Based on their C-terminal dilysine signals, Lag1p and Dgt1p should be at least partially localized to the ER membrane. Totest this prediction directly, we constructed an allele in whichthe DGT1 gene is appended with sequences encoding an N-terminalepitope derived from influenza virus HA ("HA epitope"; Field etal., 1988). This epitope-tagged protein, HA-Dgt1p, is functional,as judged by its ability to complement the growth defect of cellsdeleted for LAG1 and DGT1 (see below). Western blot controls revealedthat HA-Dgt1p was specifically recognized by monoclonal anti-HAantibodies (our unpublishedresults).

We visualized the intracellular distribution of HA-Dgt1p by indirect immunofluorescence microscopy. Cells expressing HA-Dgt1por, as a control, an untagged version of DGT1 were fixed and processedfor immunofluorescence (see MATERIALS AND METHODS). Nuclei andmitochondria were visualized using the DNA-binding dye DAPI (Figure2, B, E, and H).

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Figure 2. Immunofluorescence localization of Dgt1p to the ER. lag1 $Delta$ dgt1 $Delta$ cells harboring an HA-tagged (WBY739) or an untagged (WBY743) version of DGT1 were fixed and processed for immunofluorescence using monoclonal anti-HA (A-F) or polyclonal anti-Kar2p (G-I) antibodies followed by secondary decoration with TRITC-conjugated anti-mouse or anti-rabbit IgG. Panels show the staining pattern of TRITC to visualize HA-Dgt1p and Kar2p localization. DNA was stained with DAPI to indicate nuclei, and cells were visualized by light microscopy (phase) to observe cell morphology.

In the presence of HA-Dgt1p, anti-HA antibodies detected the characteristic yeast ER staining pattern (Figure 2A), consistingof a distinct perinuclear ring and fine strands of staining connectingthe perinuclear ER to ER cisternae underlying the plasma membrane.This pattern closely resembled that obtained in control samplesstained with polyclonal antibodies specific to the ER-lumenalprotein Kar2p (Figure 2G). Cells expressing Dgt1p without an epitopetag showed only background staining (Figure 2D). Thus HA-Dgt1p $---$ andby extension Dgt1p $---$ is localized to the ERmembrane.

Very similar results were obtained when HA-tagged alleles of LAG1 and DGT1 were overexpressed using a GAL1/10 promoter (ourunpublished results), demonstrating that both proteins are localizedto the ERmembrane.

Deletion of LAG1 and DGT1 Causes Growth Defects

As a first step toward understanding the role of Lag1p and Dgt1p, we examined the phenotypes of haploid strains deleted foreither of these genes. To this end, the entire coding regionsof LAG1 and DGT1 were replaced by the selectable marker genesHIS3 and ADE2 (see MATERIALS AND METHODS). The resulting lag1 $Delta$ and dgt1 $Delta$ null mutants grew with wild-type rates both on solidmedia and in liquid culture (Figure 3), demonstrating that neitherof these genes is essential for vegetative growth. Also, the lag1 $Delta$ and dgt1 $Delta$ mutations had no apparent effect on the shape, size,budding pattern, or viability of the cells.

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Figure 3. Lag1p and Dgt1p are important for growth. Growth rates in YPD medium of wild type and strains in which the chromosomal copies of LAG1 DGT1 or both LAG1 and DGT1 have been disrupted are shown. Growth rates were determined at 30°C as described in MATERIALS AND METHODS. Values are the average of four to six measurements; error bars indicate SD. The growth defect was observed in different rich and minimal media containing either glucose or galactose as the carbon source. When growth rates were studied on YPD at various temperatures between 15 and 40°C, lag1 $Delta$ dgt1 $Delta$ cells grew drastically slower at all temperatures tested. The growth defect was more pronounced above 35°C, indicating a slightly increased temperature sensitivity. Although lag1 $Delta$ dgt1 $Delta$ cells formed tiny colonies at 37°C, no growth was observed at 39-40°C, at which wild-type, lag1 $Delta$ , and dgt1 $Delta$ single mutant cells grew normally.

To address the possibility of overlapping functions for LAG1 and DGT1, we constructed a haploid mutant deleted for both ofthese genes. After mating of the haploid lag1 $Delta$ and dgt1 $Delta$ strains,the resulting diploid (heterozygous for both genes) was sporulated.Tetrad dissections resulted in four viable spores, most of whichgrew like wild type, whereas some grew with a significantly reducedrate. Analysis of auxotrophic markers revealed that the growthdefect cosegregated with the His⁺Ade⁺ phenotype in all 22 tetrads analyzed. In addition, genomic PCRanalysis of four colonies produced from spores of a single tetradconfirmed directly that the slowly growing His⁺Ade⁺ colonies contain the lag1 $Delta$ ::HIS3 and dgt1 $Delta$ ::ADE2 disruptions(our unpublished results). Similar to the results on agar plates,the lag1 $Delta$ dgt1 $Delta$ double mutant also showed a drastically reducedgrowth rate in liquid culture when compared with wild type andthe single disruption mutants lag1 $Delta$ and dgt1 $Delta$ (Figure 3). Takentogether, the slow-growth phenotype of the lag1 $Delta$ dgt1 $Delta$ mutantstrongly suggests an important, but not essential, function forLag1p andDgt1p.

To confirm this interpretation, we tested whether plasmids carrying genomic copies of LAG1 or DGT1 would rescue the lag1 $Delta$ dgt1 $Delta$ growth phenotype. DNA fragments containing the entire genesand their flanking sequences were subcloned into pRS316 (Sikorskiand Hieter, 1989), generating the plasmids pWB98 and pWB95. Toshow that the information contained in these DNA fragments wassufficient to complement the lag1 $Delta$ dgt1 $Delta$ null mutant, pWB98 orpWB95 was transformed into diploid cells heterozygous for bothLAG1 and DGT1. After sporulation and tetrad dissection, haploidcells bearing both chromosomal lag1 $Delta$ and dgt1 $Delta$ mutations and theplasmid were selected. By using this approach rather than transformingthe haploid lag1 $Delta$ dgt1 $Delta$ double mutant strain directly, we avoidedcomplications arising from the extremely low transformation efficiencyof lag1 $Delta$ dgt1 $Delta$ cells (see below). In all tetrads analyzed, eachHis⁺Ade⁺Ura⁺ colony (carrying both gene disruptions and the URA3-marked plasmidpWB98 or pWB95) grew at the wild-type rate. This confirms thatthese plasmids contain all the information necessary for the functionalexpression of LAG1 and DGT1.

Lag1p and Dgt1p Are Not Required for Protein Translocation across the ER Membrane

The mammalian TRAM protein is thought to be involved in protein translocation across or into the ER membrane (Do et al., 1996;Voigt et al., 1996). Because Lag1p and Dgt1p were identified throughtheir sequence similarity to the mammalian TRAM protein, we askeddirectly whether these yeast proteins play a role in protein translocationacross or membrane protein integration into the ER membrane. Tothis end, the translocation of several endogenous secretory andmembrane proteins of yeast (including SRP-dependent and -independentproteins) was assessed invivo.

Wild-type and lag1 $Delta$ dgt1 $Delta$ mutant cells were pulse labeled with [³⁵S]methionine and [³⁵S]cysteine. As a control, we used cells carrying sec61-101, amutant allele of SEC61 that impairs translocation of proteinsusing either an SRP-dependent or -independent pathway (Ng et al.,1996). Lysates from radiolabeled cells were analyzed by immunoprecipitationusing antibodies raised against proteins that are translocatedacross or integrated into the ER membrane. Defects were monitoredas the accumulation of precursor proteins lacking glycosylationand/or signal sequence cleavage, both of which occur in the ERlumen.

As shown in Figure 4A, no translocation defects were observed when lag1 $Delta$ dgt1 $Delta$ cells were analyzed using antibodies specificfor Kar2p, an ER lumenal protein (Figure 4A, lane 2). As for wild-typecells (Figure 4A, lane 1) only the translocated form of Kar2pwas observed in the mutant cells. In contrast, a significant fractionof the labeled Kar2p was recovered as the slower migrating precursorform in sec61-101 cells (Figure 4A, lane 3; the slower mobilityof preKar2p in SDS-PAGE represents the presence of an uncleavedsignal sequence), as was observed previously (Ng et al., 1996).

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Figure 4. Protein translocation across the ER membrane does not require LAG1 and DGT1. Cells of W303-1B (wild type), WBY616 (lag1 $Delta$ dgt1 $Delta$ ), or DNY116 (sec61-101) were pulse labeled with [³⁵S]methionine and [³⁵S]cysteine for 5 min. Cell lysates were prepared, and immunoprecipitations were performed using polyclonal antibodies against the following proteins: (A) Kar2p, (B) dipeptidyl aminopeptidase B (DPAP B), (C) CPY, and (D) the GPI-anchored cell surface protein Gas1p. Eluates were subjected to SDS-PAGE followed by fluorography. Cytosolic precursor (p) and ER-glycosylated (g) forms of each protein are indicated.

Similar results were obtained for all other proteins tested. In particular, dipeptidyl aminopeptidase B (a vacuolar type IIintegral membrane protein; Figure 4B), carboxypeptidase Y (CPY,a soluble vacuolar protein; Figure 4C), Gas1p (a cell surfaceglycoprotein; Figure 4D), $alpha$ -factor (a secreted yeast pheromone),protein disulfide isomerase (an ER-lumenal protein), and Pho8p(a type II integral membrane protein; our unpublished results)showed no evidence of translocation defects in lag1 $Delta$ dgt1 $Delta$ cells.Because translocation or membrane integration of this broad spectrumof proteins was not affected by the deletion of LAG1 and DGT1,these genes are unlikely to play a general role in proteintranslocation.

Deletion of LAG1 and DGT1 Causes Cell Wall Defects

Attempts to transform the haploid lag1 $Delta$ dgt1 $Delta$ mutant with plasmids revealed that the deletion of these genes caused severedefects in transformation efficiency. Only very few transformantswere obtained with either of two standard transformation procedures,using lithium acetate or electroporation. A quantitative analysisof this phenomenon is shown in Figure 5. When exponentially growingcells from wild-type or the single null mutants (lag1 $Delta$ or dgt1 $Delta$ )were transformed using lithium acetate, we obtained transformationrates of ~10⁵ transformants/µg of plasmid DNA. In contrast, the transformationefficiency of lag1 $Delta$ dgt1 $Delta$ cells was reduced by greater than fourorders of magnitude. Although the addition of pWB96 (carryingDGT1) resulted in the transformation of a few lag1 $Delta$ dgt1 $Delta$ cells,not a single transformant was obtained with the control vectorpRS314 (Figure 5). Additional experiments revealed that lag1 $Delta$ dgt1 $Delta$ cells gave rise to a drastically lower number of coloniesthan wild-type cells even when the transformation mixtures wereplated on YPD plates instead of selective plates. Thus, the transformationprocedure per se appeared to be lethal to lag1 $Delta$ dgt1 $Delta$ cells. Furthercharacterization of the transformation procedure demonstratedthat the death of lag1 $Delta$ dgt1 $Delta$ cells was primarily caused by thestep involving treatment with DMSO and 42°C heat shock (our unpublishedresults), suggesting that the deletion of LAG1 and DGT1 generallydestabilizes the cells possibly by impairing cell wall integrity.

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Figure 5. The transformation efficiency of lag1 $Delta$ dgt1 $Delta$ cells is drastically impaired. Yeast cells were grown at 30°C in YPD medium to logarithmic phase (OD₆₀₀ = 0.4-0.6), and 0.5 OD₆₀₀ cell equivalents were transformed with 3 µg of a plasmid with (pWB96; hatched bars) or without (pRS314; black bars) DGT1. Dilutions of the samples were plated onto selective minimal plates, and transformation rates were determined from the number of TRP⁺ colonies.

To determine directly whether the lag1 $Delta$ dgt1 $Delta$ mutant exhibited any ultrastructural changes indicative of cell wall defects,thin sections of the different mutants were studied by electronmicroscopy. Figure 6, B and C, shows that lag1 $Delta$ and dgt1 $Delta$ cellsare morphologically indistinguishable from wild-type cells (Figure6A). In contrast to the single disruption mutants, the lag1 $Delta$ dgt1 $Delta$ double mutants have severe cell wall defects (Figure 6, D-F).Normal cell walls were observed as a single electron translucentcentral layer, composed largely of $beta$ -glucan, which is surroundedby an electron-dense shell of mannoproteins (for review, see Klis,1994). In contrast, lag1 $Delta$ dgt1 $Delta$ cell walls show several distinctlayers (Figure 6, D-F, arrowheads), each with a thickness aboutthat of a normal cell wall, suggesting that they are built throughrepeated deposition of cell wall material. Most of the lag1 $Delta$ dgt1 $Delta$ cells observed have cell walls that were drastically thicker (upto 500 nm) than the wild-type cell wall (150-200 nm). In somesections of lag1 $Delta$ dgt1 $Delta$ cells, budding daughter cells could beobserved that were still attached to their mother cells (Figure6D). Interestingly, in these images, the growing bud exhibiteda relatively normal cell wall morphology. The inner cell walllayer of the mother cell appeared to be continuous with the cellwall of the bud, whereas the extra outer wall layers of the mothercell ended at the septum (Figure 6D, arrows).

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Figure 6. Altered cell wall morphology of the lag1 $Delta$ dgt1 $Delta$ mutant. Cells were grown in YPD medium at 30°C and fixed with permanganate, and thin sections were prepared for electron microscopy as described in MATERIALS AND METHODS. (A) Wild-type (W303-1A), (B) lag1 $Delta$ (WBY283), (C) dgt1 $Delta$ (WBY286), (D-F) lag1 $Delta$ dgt1 $Delta$ (WBY616). N, nucleus; V, vacuole. Note the thick, multilayered cell wall on lag1 $Delta$ dgt1 $Delta$ mother cells.

Several mutants with cell wall defects have been shown to grow at a reduced rate unless the medium is osmotically supportedwith 1 M sorbitol (Levin and Bartlett-Heubusch, 1992). However,the growth defect of lag1 $Delta$ dgt1 $Delta$ cells was not rescued by theaddition of 1 M sorbitol to the growth medium (our unpublishedresults), excluding the possibility of an osmotic hypersensitivityof the lag1 $Delta$ dgt1 $Delta$ cells.

The aberrant cell wall structure of the lag1 $Delta$ dgt1 $Delta$ mutant may explain the drastically impaired transformation efficiency(Figure 5) and suggested that Lag1p and Dgt1p are involved, directlyor indirectly, in some process related to cell wallbiogenesis.

LAG1 and DGT1 Facilitate ER-to-Golgi Transport of GPI Proteins

The results presented above show that Lag1p and Dgt1p are localized to the ER membrane and are required for proper cell wallformation. Yet we could not obtain evidence that Lag1p or Dgt1pare involved in protein translocation, as originally suggestedby their sequence similarity to mammalian TRAM. Because cell walldefects could, in principle, arise from an impaired delivery ofsome proteins to the cell surface, we addressed the possibilitythat Lag1p or Dgt1p might play a role in protein trafficking beyondthe ER, such as from the ER to the Golgi compartment. To thisend, we assessed the maturation kinetics of several marker proteinsusing pulse-chase analysis, followed by immunoprecipitation andSDS-PAGE analysis (Figure 7).

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Figure 7. Maturation of Gas1p and Yap3p, but not CPY and Pho8p, is defective in lag1 $Delta$ dgt1 $Delta$ cells. The rate of conversion of the precursor forms of CPY, Pho8p, Gas1p, or Yap3p to their mature products was determined by pulse labeling cells for 2 min with [³⁵S]methionine and [³⁵S]cysteine followed by a chase with an excess of unlabeled methionine and cysteine. At the indicated times, cell extracts of wild-type (wt) or lag1 $Delta$ dgt1 $Delta$ ( $Delta$ $Delta$ ) cells were made, and immunoprecipitations were performed using antibodies against CPY (A), Pho8p (B), Gas1p (C), or Yap3p (D). Eluates were subjected to SDS-PAGE followed by autoradiography. Precursor and mature (m) forms of each protein are indicated, ER-glycosylated and Golgi-modified forms of CPY are labeled p1 and p2, respectively. The graphs shown on the right indicate the percentages of mature proteins (determined by quantitating the radioactivity in the relevant bands using a PhosphorImager). Values are the average of three measurements; error bars indicate SD. Triangles, W303 (wild-type); diamonds, WBY283 (lag1 $Delta$ ); circles, WBY616 (lag1 $Delta$ dgt1 $Delta$ ); square, NY414 (sec13-1). Open symbols indicate experiments performed at 30°C, closed symbols represent results obtained at 37°C.

First, we studied the biogenesis of CPY, a vacuolar enzyme. The results in Figure 7A show that the maturation kinetics ofCPY are indistinguishable in wild-type and lag1 $Delta$ dgt1 $Delta$ cells.The 67-kDa ER form (Figure 7A, p1) of CPY is rapidly convertedto the 69-kDa Golgi form (Figure 7A, p2), which in turn is proteolyticallycleaved in the vacuole to the 61-kDa mature form (Figure 7A, mCPY)(Stevens et al., 1982). These data demonstrate that the absenceof Lag1p and Dgt1p does not delay ER-to-Golgi transport of CPY.Similar results were obtained using antibodies against Pho8p,a vacuolar type II integral membrane protein (Figure 7B). The74-kDa ER precursor form of Pho8p is proteolytically cleaved inthe vacuole to the 72-kDa mature form (Klionski and Emr, 1989).Because CPY and Pho8p maturation are indicative of vacuolar delivery,we conclude that Lag1p and Dgt1p do not play an important rolein the general protein transportpathway.

Next, we addressed the possibility that these proteins might be involved in the vesicular transport of a specific subset ofproteins (such as cell wall proteins). Specifically, we studiedthe maturation of GPI-anchored proteins, a group of cell surfaceproteins carrying a C-terminal lipid anchor that becomes attachedonto specific proteins in the ER (Takeda and Kinoshita, 1995).The ER-to-Golgi transport of GPI proteins is dependent on theaddition of the GPI anchor (Nuoffer et al., 1991; Doering andSchekman, 1996). Because Lag1p and Dgt1p are localized to theER membrane, they might be required for GPI anchor attachmentsor the transport of GPI proteins. To address this possibility,we analyzed the ER-to-Golgi transport of Gas1p, a well-characterizedGPI model protein (Nuoffer et al., 1991). Vesicular transportof Gas1p can be monitored by following the conversion of the 105-kDacore-glycosylated ER form to the 125-kDa mature form, which isformed upon arrival in the Golgi compartment (Fankhauser and Conzelmann,1991; Nuoffer et al. 1991, 1993). When Gas1p does not receivea GPI anchor in the ER, it is not efficiently transported to theGolgi apparatus and remains in its immature 105-kDa form (Nuofferet al., 1993; Doering and Schekman, 1996).

The maturation of Gas1p was examined in wild-type and the different disruption mutants using pulse-chase analysis, followedby immunoprecipitation and SDS-PAGE analysis (Figure 7C). As acontrol, we used a temperature-sensitive secretion mutant (sec13-1;Novick et al., 1980, 1981) in which the vesicle traffic is completelyblocked between the ER and the Golgi apparatus (Figure 7C, filledsquare). As observed before, the maturation of Gas1p is rapidin wild-type cells, with a half-time of ~10 min (Hamburger etal., 1995; Schimmöller et al., 1995; Sütterlin et al., 1997).Very similar results were obtained using the individual deletionmutants lag1 $Delta$ (Figure 7C) and dgt1 $Delta$ (our unpublished results).In lag1 $Delta$ dgt1 $Delta$ cells, however, maturation of Gas1p was significantlydelayed with a half-time of ~20 min (observed at both 30 and 37°C).

Quantitative analysis of the data (Figure 7C, right) indicates that even in the absence of LAG1 and DGT1 most of Gas1p waspresent in the mature Golgi form after a 30-min chase. At theselater time points, however, we consistently observed a significantloss of the total Gas1p signal, suggesting that a significantportion of the unmature Gas1p molecules were being degraded. Thiseffect may not reflect a phenotype resulting from the disruptionof LAG1 and DGT1, however, because Gas1p matured equally inefficientlyin wild-type cells (Figure 7C, wild-typecontrol).

The delayed maturation of Gas1p observed in the lag1 $Delta$ dgt1 $Delta$ mutant suggests that Lag1p and Dgt1p may be required for efficientER-to-Golgi transport of GPI-anchored proteins in general. Totest this notion, we investigated the maturation kinetics of anotherGPI-protein, the aspartyl endoprotease Yap3p. Pulse-chase-labeledprotein extracts were immunoprecipitated using anti-Yap3p antibodies(Ash et al., 1995). As shown in Figure 7D, two different proteinsof 80 and 100 kDa were precipitated at early time points. Thesebands presumably correspond to differently core-glycosylated ERforms of Yap3p, because both can be converted to a single bandof ~70 kDa upon treatment with endoglycosidase H (our unpublishedresults). At later time points, hyperglycosylated Yap3p is formed,which migrates as a broad band on SDS polyacrylamide gels at ~160kDa and is indicative of the protein's arrival in the Golgi apparatus(Ash et al., 1995).

We quantitated the amount of both ER forms as well as the 160-kDa Golgi form of Yap3p to measure the relative block in ER-to-Golgitransport. As shown in Figure 7D, right, the hyperglycosylatedGolgi form of Yap3p was formed with a half-time of ~5 min in wild-typecells. In contrast, Yap3p maturation was delayed in lag1 $Delta$ dgt1 $Delta$ cells (half-time, 8-9 min). Although this difference was lesspronounced than for Gas1p, it was reproduced in three separateexperiments (the average values and SDs are shown in Figure 7D).Thus, we conclude that Lag1p and Dgt1p facilitate efficient ER-to-Golgitransport ofYap3p.

GPI Anchor Attachment Is Not Defective in the lag1 $Delta$ dgt1 $Delta$ Mutant

Taken together, the results presented thus far show that the loss of Lag1p and Dgt1p causes a delay in the maturation of GPI-anchoredproteins, whereas the vesicular transport of other proteins suchas CPY and Pho8p occurs with wild-type kinetics. Thus, the phenotypeof lag1 $Delta$ dgt1 $Delta$ is quite distinct from sec mutants, which completelyblock the secretory pathway. One possible explanation for theobserved cargo specificity of the transport defect would be thatGPI anchor attachment is defective in the lag1 $Delta$ dgt1 $Delta$ mutant.Indeed, a temperature-sensitive mutation of GAA1, encoding a proteininvolved in GPI anchor attachment, causes a similar delay in theER-to-Golgi transport of Gas1p (Hamburger et al., 1995).

To test this possibility, we labeled cells with [³H]-myo-inositol, a biosynthetic precursor of the GPI anchor that becomesincorporated into the whole spectrum of GPI-anchored proteins(Conzelmann et al., 1990), and compared the rates of GPI anchorattachment in wild-type and lag1 $Delta$ dgt1 $Delta$ cells. As a control, weused a strain carrying a temperature-sensitive allele of GAA1,gaa1-1 (Hamburger et al., 1995).

The incorporation of [³H]myo-inositol into proteins was analyzed by labeling wild-type, lag1 $Delta$ dgt1 $Delta$ , and gaa1-1 cells for differentlengths of time. Total protein extracts were prepared and delipidated,and the GPI proteins were visualized by SDS-PAGE and fluorography.As shown in Figure 8, lanes 1-3, wild-type cells incorporated[³H]inositol into a distinct pattern of bands reminiscent of thatobserved before (Hamburger et al., 1995; Schönbächler et al.,1995). Interestingly, the pattern of [³H]inositol-labeled proteins in wild-type cells closely resembledthat of lag1 $Delta$ dgt1 $Delta$ mutant cells, indicating that all abundantGPI proteins were correctly modified in the absence of Lag1p andDgt1p (Figure 8, lanes 1-6). Furthermore, the kinetics of [³H]-inositol incorporation were similar in both strains, demonstratingthat Lag1p and Dgt1p are not required for the efficiency of GPIanchor biosynthesis and attachment. Because the banding patternin the wild-type and lag1 $Delta$ dgt1 $Delta$ strains is indistinguishable,the kinetic delay in GPI-anchored protein maturation (see Figure7) can only have a minor effect on the majority of the monitoredproteins, because otherwise maturation intermediates with differentmobilities should have been observed. As observed before (Hamburgeret al., 1995), inositol incorporation into proteins was almostcompletely abolished in the gaa1-1 mutant (Figure 8, lanes 7-9).

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Figure 8. GPI anchor attachment does not require LAG1 and DGT1. Wild-type (wt), WBY616 (lag1 $Delta$ dgt1 $Delta$ ), or RH2856 (gaa1-1) cells were preincubated for 5 min and pulse labeled with [³H]myo-inositol for the indicated times at 30°C, except for RH2856, which was preincubated and labeled at 37°C. Total protein extracts were prepared, delipidated, and separated by SDS-PAGE followed by fluorography at $-$ 70°C.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

We have identified and characterized two ER transmembrane proteins that are members of an evolutionarily conserved familyand, at least in yeast, appear to be involved in ER-to-Golgi transportof GPI-anchored proteins. This conclusion is suggested by theobservation that the deletion of LAG1 and DGT1 delays the maturationof two GPI-anchored proteins, for which we have determined theER-to-Golgi transport kinetics (Figure 7), but does not impairor delay the attachment of GPI anchors in general (Figure 8).The transport defect is only observed in the lag1 $Delta$ dgt1 $Delta$ doublemutant but not in strains individually deleted for LAG1 or DGT1,suggesting redundant or overlapping functions for these gene products.Because the ER-to-Golgi transport of GPI-anchored proteins isonly partially impaired in lag1 $Delta$ dgt1 $Delta$ cells, Lag1p and Dgt1pfacilitate, but are not essential, for the transport of GPI-anchoredproteins.

Possible Roles of Lag1p and Dgt1p in GPI-anchored Protein Transport

One possible function of Lag1p and Dgt1p is to serve as "escortins" that directly interact with and facilitate movement ofGPI-anchored proteins out of the ER. In addition to mutationsthat impair GPI anchoring, deletion of EMP24 or ERV25, two genesencoding transmembrane proteins that are enriched in COPII transportvesicles, also delays the maturation of a subset of proteins,including Gas1p but also other, non-GPI-anchored proteins (Schimmölleret al., 1995; Belden and Barlowe, 1996). These proteins belongto the p24 class of type I membrane proteins that were proposedto serve as selective "cargo receptors" in the sorting and packagingof proteins into COPII vesicles (Fiedler et al., 1996; Sohn etal., 1996). Because cargo recruitment from the ER is thought toinvolve selective mechanisms, it is conceivable that Lag1p andDgt1p serve as "GPI receptors," possibly in collaboration withEmp24p and Erv25p, in selectively packaging of GPI-anchored proteinsinto transportvesicles.

The presence of ER retention signals in Lag1p and Dgt1p supports this interpretation. The KKXX signal is recognized by COPI,which is thought to be involved in recycling from the Golgi compartment(Letourneur et al., 1994). This suggests that Lag1p and Dgt1pcycle between the ER and Golgi, which would be an essential aspectof the function of cargo receptors that become copackaged intothe transport vesicles. This view would also be consistent withthe recent observation that the ER-to-Golgi transport of GPI-anchoredproteins is selectively blocked in ret1-1, a mutant in the $alpha$ -subunitof COPI (Sütterlin, et al., 1997). Because the primary role ofCOPI is thought to be the retrieval of proteins from the Golgito the ER (Letourneur et al., 1994; Lewis and Pelham, 1996), thisresult suggests that cycling of component(s) involved in GPI-anchoredprotein transport is required. It remains to be shown whetherLag1p and Dgt1p cycle between the ER and Golgi. Alternatively,they could reside permanently in the ER, with the KKXX retrievalsignal only providing a backup function to retrieve those moleculesthat have inappropriately escaped the ER.

Another possibility is that Lag1p and Dgt1p affect GPI-anchored protein maturation more indirectly. A reduced rate of GPI-anchoredprotein transport was also observed, for example, when the biosynthesisof sphingolipids was blocked either by treatment with myriocin,an inhibitor of ceramide synthesis (Horvath et al., 1994), orby a mutation in LCB1, encoding the first enzyme in sphingolipidbiosynthesis (Sütterlin et al., 1997). Interestingly, this mutationalso affects Gas1p and Yap3p transport to quantitatively differentdegrees, as we observed in Figure 7.

Thus, ER-to-Golgi transport of GPI proteins is dependent on sphingolipid synthesis, indicating that sphingolipids might interactwith GPI proteins to initiate transport. Studies in polarizedepithelial cells have shown that GPI-anchored proteins and sphingolipidsare cotransported from the Golgi to the apical plasma membrane,suggesting that GPI proteins and sphingolipids associate to formmicrodomains, or "rafts," in the trans-Golgi network, which arethen recruited into vesicles bound for the apical surface (Simonsand van Meer, 1988; Brown and Rose, 1992). The GPI anchor allowsGPI-anchored proteins to enter such domains, from which othersecretory proteins are excluded. A similar "clustering hypothesis"has been proposed in yeast, where ER-to-Golgi transport of GPI-anchoredproteins seems to depend on their interaction with sphingolipids.Therefore, sphingolipids may stimulate the clustering of GPI proteinsas a prelude to their packaging into specific transport vesicles(Horvath et al., 1994; Skrzypek et al., 1997) or facilitate thefusion of GPI-containing vesicles with the Golgi membrane (Sütterlinet al., 1997). Deletion of Lag1p and Dgt1p could therefore impairthe biogenesis or availability of sphingolipids and hence delaymaturation of GPI-anchored proteins moreindirectly.

Clearly, other models could also explain the results obtained in this study. For example, Lag1p and Dgt1p could serve as molecularchaperones for the folding or assembly of GPI-anchored proteinsimmediately after GPI anchor attachment. Future studies will benecessary to distinguish between these conceptually distinctpossibilities.

Relationship to the Longevity Phenotype of lag1 $Delta$ Cells

LAG1 (for "longevity-assurance gene 1") has been described previously to play a role in regulating life span and aging inyeast (D'mello et al., 1994). In that study, LAG1 was found tobe differentially expressed during the cell's replicative lifespan, i.e., predominantly in younger cells. Furthermore, a mutantdisrupted for LAG1 displayed a drastically increased life span,i.e., an increased average number of cell divisions performedby an individual cell (D'mello et al., 1994). The molecular causefor this increase in life span has not been described. However,the "longevity phenotype" was described for a lag1 $Delta$ single disruption,whereas the GPI transport phenotype was only observed after disruptionof both LAG1 and DGT1. Therefore, we consider a direct link betweenthese two phenotypes veryunlikely.

Sequence Similarities to Mammalian Proteins

Although we initiated our studies of Lag1p and Dgt1p because of their sequence similarity to mammalian TRAM proteins, theseproteins appear functionally distinct. Several studies have shownthat TRAM is intimately associated with protein translocationacross and integration into the ER membrane. In particular, TRAMwas shown 1) to be required for the translocation of most butnot all proteins (Görlich et al., 1992; Voigt et al., 1996),2) to be in close proximity to the signal sequence during earlyphases of translocation (High et al., 1993; Mothes et al., 1994),3) to be involved in the formation of a tight ribosome-membranejunction early in translocation (Voigt et al., 1996), 4) to interactwith a transmembrane segment during its membrane integration (Doet al., 1996), and 5) to play a role in regulating "translocationalpausing," a mechanism by which certain nascent secretory proteinsare transiently exposed to the cytosol (Hegde et al., 1998). Allthese results suggest that TRAM is stoichiometrically associatedwith the translocon and is involved in facilitating and/or regulatingsome aspect of the translocation-integration process perse.

In contrast, our results demonstrate that the yeast proteins Lag1p and Dgt1p play a different molecular role. Because allseven substrates tested (including soluble and membrane proteinsas well as SRP-dependent and -independent proteins) are translocatednormally in the lag1 $Delta$ dgt1 $Delta$ mutant, we conclude that Lag1p andDgt1p are not involved in protein translocation and integration.Formally, however, we cannot rule out the possibility that someother, still unidentified protein(s) require(s) Lag1p and Dgt1pat the stage of membrane translocation or integration into theER. Thus it appears that mammalian TRAM and yeast Lag1p and Dgt1phave a common evolutionary origin, but their functions have diverged.Because Lag1p and Dgt1p also show a similar degree of sequencesimilarity (~20% identity over the entire length) to the productsof two other mammalian genes of unknown function, KIAA0057 (Nomuraet al., 1994) and UOG1 (Lee, 1991), it is possible that one orboth of them perform a similar role in GPI transport as Lag1pandDgt1p.

Cell Wall Defects

The pronounced cell wall defects in lag1 $Delta$ dgt1 $Delta$ cells are characterized by an extremely low efficiency of plasmid transformationand by thickened, multilayered cell walls (Figures 5 and 6). Cellwall thickening was only detected in mother cells, whereas mostbuds display normal cell wall thickness. These results suggestthat the mutant walls are built through repeated deposition ofcell wall material, possibly as the result of feedback regulationthat continually tries to correct earlierdefects.

Two lines of evidence underline the importance of GPI-anchored proteins for cell wall integrity. First, mutations that affectdifferent steps of the GPI biosynthesis show increased sensitivitiesto calcofluor white and hygromycin B (Benghezal et al., 1995;Vossen et al., 1995, 1997), which are characteristic of defectsin cell wall integrity. Consistent with this observation, lag1 $Delta$ dgt1 $Delta$ cells are hypersensitive to calcofluor white and hygromycinB (our unpublished results). Second, GPI-anchored proteins areknown to play an important role in covalently cross-linking cellwall proteins to the cell wall glucan (Lu et al., 1995; Roemerand Bussey, 1995). Therefore, perturbation of the GPI pathwaymight change the rate of cell wall construction, possibly causingaberrant covalent binding or secretion of cell wall proteins.The deletion of the GPI-anchoring signal of agglutinin $alpha$ , forexample, prevents its incorporation into the cell wall and resultsin its secretion as an inactive molecule into the medium (Wojciechowiczet al., 1993). Also, a mutant in GPI3, a gene involved in thefirst step of GPI synthesis, produces only very limited amountsof GPI anchors, thus causing accumulation of ER precursors ofGPI-dependent cell wall proteins (Vossen et al., 1997). The majorityof cell wall proteins that eventually leave the ER of this mutantare not covalently incorporated into the cell wall but are secretedinto the growth medium, indicating that improper delivery of GPI-anchoredproteins can have profound effects on the proper incorporationof cell wall proteins. In gpi3 mutants, however, no thickeningof the cell wall was apparent when they were analyzed at semipermissivetemperature (Vossen et al., 1997). Although we do not understandthe molecular differences that are responsible for the differencesin cell wall morphology, it remains plausible that the observedkinetic retardation of GPI-anchored protein transport in lag1 $Delta$ dgt1 $Delta$ mutant cells accounts for the observed cell walldefects.

Similarly, the growth defect of lag1 $Delta$ dgt1 $Delta$ cells can also be explained by an impaired transport of GPI-anchored proteins.All GPI pathway mutants have lower growth rates compared withwild type (Benghezal et al., 1995; Hamburger et al., 1995; Vossenet al., 1997). Furthermore, growth is impaired if the synthesisor attachment of GPI anchors is selectively blocked by depletionof inositol (Doering and Schekman, 1996) or by alteration of theGPI-anchoring signal of Gas1p (Nuoffer et al., 1991). Our resultsare therefore consistent with the view that the availability ofGPI proteins is a limiting factor in cell wall construction andgrowth.

	ACKNOWLEDGMENTS

We are grateful to Sandra Huling for taking the electron micrographs and to Rita Wiemeyer for excellent technical assistance.We thank A. Conzelmann for antibodies against Gas1p, Y. Bourbonnaisfor antibodies against Yap3p, and H. Riezman for the gaa1-1 mutantstrain RH2856. We also thank Corinna Barz, Ted Powers, and StefanSchorling for helpful discussions and D. Oesterhelt for support.This work was supported by a research fellowship from the DeutscheForschungsgemeinschaft to W.P.B. and by grants from the NationalInstitutes of Health to P.W. P.W. is an Investigator of the HowardHughes MedicalInstitute.

	FOOTNOTES

Corresponding author. E-mail address: barz{at}biochem.mpg.de.

ABBREVIATIONS

Abbreviations used: bp, base pair; COP, coatomer protein; CPY, carboxypeptidase Y; ER, endoplasmic reticulum; GPI, glycosylphosphatidylinositol; HA, hemagglutinin; Ig, immunoglobulin; kb, kilobase; SRP, signal recognition particle; SC, synthetic complete; TRAM, translocating chain-associated membrane protein.

	REFERENCES

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

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