ER-Golgi Traffic Is a Prerequisite for Efficient ER Degradation

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Originally published as MBC in Press, 10.1091/mbc.01-08-0399 on April 3, 2002

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Vol. 13, Issue 6, 1806-1818, June 2002

ER-Golgi Traffic Is a Prerequisite for Efficient ER Degradation

Christof Taxis,^* Frank Vogel, and Dieter H. Wolf^*

^*Institut für Biochemie, Universität Stuttgart, 70569 Stuttgart, Germany; and Max-Delbrück-Centrum für Molekulare Medizin, 13125 Berlin, Germany

Submitted August 9, 2001; Revised February 19, 2002; Accepted February 22, 2002
Monitoring Editor: Howard Riezman

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Protein quality control is an essential function of the endoplasmic reticulum. Misfolded proteins unable to acquire theirnative conformation are retained in the endoplasmic reticulum,retro-translocated back into the cytosol, and degraded via theubiquitin-proteasome system. We show that efficient degradationof soluble malfolded proteins in yeast requires a fully competentearly secretory pathway. Mutations in proteins essential for ER-Golgiprotein traffic severely inhibit ER degradation of the model substrateCPY*. We found ER localization of CPY* in WT cells, but no otherspecific organelle for ER degradation could be identified by electronmicroscopy studies. Because CPY* is degraded in COPI coat mutants,only a minor fraction of CPY* or of a proteinaceous factor requiredfor degradation seems to enter the recycling pathway between ERand Golgi. Therefore, we propose that the disorganized structureof the ER and/or the mislocalization of Kar2p, observed in earlysecretory mutants, is responsible for the reduction in CPY* degradation.Further, we observed that mutations in proteins directly involvedin degradation of malfolded proteins (Der1p, Der3/Hrd1p, and Hrd3p)lead to morphological changes of the endoplasmic reticulum andthe Golgi, escape of CPY* into the secretory pathway and a slowermaturation rate of wild-typeCPY.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Protein quality control with subsequent elimination of malfolded proteins or unassembled subunits is essential for cellularfunction. Disturbed quality control leads to disease and eventuallyto cell death (Plemper and Wolf, 1999; Kopito and Sitia, 2000).The endoplasmic reticulum (ER) is the folding compartment forproteins destined to function within the ER itself and for secretoryproteins of the Golgi, endosomes, vacuoles, and plasma membraneas well as for proteins secreted extracellularly. It containsa multitude of folding enzymes and chaperones to perform thisfunction (Ellgaard et al., 1999; Zapun et al., 1999). Failurein folding or in the assembly of multimeric complexes leads torecognition by the quality control machinery in the ER. The proteinsare then transported back into the cytoplasm, most likely viathe Sec61 translocon, and degraded by the ubiquitin-proteasomesystem (Kopito, 1997; Sommer and Wolf, 1997; Brodsky and McCracken,1999; Plemper and Wolf, 1999). Polyubiquitination is mediatedthrough the action of the E2 enzymes, Ubc1p and Ubc7p, and themembrane bound RING-H2 ubiquitin-protein ligase (E3) Der3/Hrd1p,which is complexed to another membrane protein, Hrd3p (Hilleret al., 1996; Plemper et al., 1999; Friedländer et al., 2000;Gardner et al., 2000; Bays et al., 2001a; Deak and Wolf, 2001).The final degradation is carried out by the proteasome, a multicatalyticand multifunctional proteinase machinery (Hilt and Wolf, 2000).Depending on the nature of the malfolded substrate protein, additionalcomponents of the ubiquitination machinery (i.e., the ubiquitinconjugating enzyme [E2 Ubc6p; Biederer et al., 1996; Hiller etal., 1996) and of the lumenal ER folding machinery (the Hsp70chaperone Kar2p, protein-disulfide isomerase [PDI], $alpha$ -1,2 mannosidase,the lectin-like protein Mnl1/Htm1 (Knop et al., 1996b; Plemperet al., 1997; Brodsky et al., 1999; Gillece et al., 1999; Jakobet al., 2001; Nakatsukasa et al., 2001) or an ER membrane proteinof unknown function (Der1p; Knop et al., 1996a) are required forthe degradationevent.

We had previously shown that a defect in ERD1, involved in the retrieval of HDEL-containing proteins from the Golgi to theER (Hardwick et al., 1990), leads to the escape of CPY* from theER, despite the fact that CPY* does not contain the HDEL retrievalsequence (Knop et al., 1996a). We were, therefore, interestedin the question whether the secretory competence of the ER ingeneral is necessary for the degradation of malfolded proteins.Intracellular transport of proteins is mediated by coated vesicles:proteins are packed into COPII-coated vesicles at ER exit sitesand transported to the Golgi apparatus, where they fuse with thetarget membrane (Rothman and Wieland, 1996; Schekman and Orci,1996; Kuehn et al., 1998). On arrival at the Golgi complex proteinsare sorted to the peripheral compartments of the cell such asvacuoles, plasma membrane, and secretory vesicles. Proteins canalso be retrieved to the ER by retrograde transport from eitherthe ER-Golgi intermediate compartment or the Golgi complex itself,by COPI-coated vesicles (Letourneur et al., 1994; Allan and Balch,1999).

It has been previously shown that extensive protein misfolding and accumulation in the ER activates the unfolded protein response(UPR; Knop et al., 1996a; Chapman et al., 1998; Casagrande etal., 2000; Friedländer et al., 2000; Travers et al., 2000). Signalingof malfolded proteins in the ER occurs via Ire1p, a kinase/nucleaseof the ER and the nuclear envelope, which activates the transcriptionfactor Hac1p. This activation leads to transcriptional upregulationof genes necessary to relieve the cell from ER stress (Chapmanet al., 1998). As one might expect, genes involved in ER degradationdirectly, such as DER1, DER3/HRD1, HRD3, and UBC7 are targetsof Hac1p (Travers et al., 2000). Furthermore, transcription ofgenes involved in ER-to-Golgi trafficking, protein targeting tothe vacuole and the cell surface, lipid metabolism, and glycosylationare also upregulated upon ER stress (Travers et al., 2000). Inthis study, we investigated the requirement of a fully operationalearly secretory pathway and a competent UPR for efficient ER degradation.As a soluble model substrate of ER degradation in yeast we examinedthe disappearance of malfolded carboxypeptidase yscY (CPY*; Fingeret al., 1993; Hiller et al., 1996; Knop et al., 1996a). In addition,we tested the influence of defective ER degradation on the secretorysystem.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Construction and Growth Conditions of Strains

Previously described standard methods were used in media preparation and for genetic and molecular biological techniques (Guthrieand Fink, 1991; Ausubel, 1992). The Saccharomyces cerevisiae strainsused in this study are summarized in Table 1. Yeast cells weregrown at 25°C (temperature-sensitive strains) or 30°C. For generationof the ufe1-1 integration plasmid, pUT1 (Lewis et al., 1997),containing the ufe1-1 allele, was digested with SalI and SpeI,and the 1450 base-pair ufe1-1 fragment was ligated into pRS306(Sikorski and Hieter, 1989) to obtain pCT27. SnaBI linearizedpCT27 was used to replace the chromosomal UFE1 allele by two-stepgene replacement (Scherer and Davis, 1979). RSY281 (sec23-1; Kaiserand Schekman, 1990), CBY263 (sed5-1; Cao et al., 1998), and RSY277(sec21-1; Letourneur et al., 1994) were backcrossed multiple timesthrough W303-1C or YCT458 to obtain the isogenic strains YCT441,YCT480, and YCT611, respectively. The IRE1 gene was deleted usingplasmid pJU341, containing the IRE1 knock out fragment (Friedländeret al., 2000). Crossing of the respective single mutants to eachother produced the double-mutant strains YCT541 and YCT542. Toobtain strains YCT458, YCT462, YCT460, YCT437, and YCT438, BglIIlinearized plasmid pRS306prc1-1 (Knop et al., 1996a) was usedto introduce the prc1-1 allele into strains YR1070 (wild-type),YR1068 (sec12-1), YR1069 (sec18-1; H. Rudolph), RH448 (wild-type),and RH2688 (sec27-1; Schröder-Köhne et al., 1998) using two-stepgene replacement (Scherer and Davis, 1979). YCT614 was generatedfrom strain YCT438 by deleting the PEP4 gene with PvuII-digestedpWO139. Integration was confirmed by Southern blotting. PlasmidpWO139 was generated through ligation of the 1.1-kb URA3 containingan EcoRI/SmaI fragment from Yep24 (Botstein et al., 1979) intoEcoRI/MscI digested plasmid pWO261. For generation of plasmidpWO261 a 1.9-kb SacI/XhoI fragment from pTZ18 (Rupp and Wolf,1995), containing PEP4, was ligated into pBluescript KS⁺ (Stratagene, La Jolla, CA).

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Table 1. Yeast strains used in this study

To express CPY*-HA, we fused prc1-1HA behind the TDH3 (pCT43) or CUP1 (pCT52) promoter. Similarly, PRC1 was fused behind theTDH3 promoter (pCT70) for expression of CPY. The cloning strategyto obtain plasmids pCT41, pCT43, pCT52, and pCT70 is availableon request. The yeast strain bearing the prc1-1HA allele was obtainedaccording to M. Longtine (Longtine et al., 1998) using plasmidpFA6a-3HA-kanMX6. For generation of plasmid pWO152, a 3-kb BamHI/HindIIIfragment, containing SEC18, was ligated into pRS426 (Christiansonet al., 1992).

Pulse-chase Analysis

Yeast strains were grown logarithmically in CM medium and labeled for 20 min with ³⁵S-methionine (pulse). Temperature-sensitive strains were shiftedto 37°C for the times indicated in legends to figures. After additionof an excess of nonradioactive methionine, samples were takenat the indicated time points. Cell disruption, immunoprecipitation,and SDS-PAGE were performed as previously described (Plemper etal., 1999). Curves were generated plotting the mean values oftwo to four independent experiments. Maturation analysis of CPYand proteinase yscA (PrA) was performed similarly, except thatthe strains were labeled for only 5min.

Electron Microscopy

For immuno-electron microscopy (EM), cells were fixed in a mixture of freshly prepared 4% formaldehyde and 0.5% glutaraldehydein 0.1 M citrate buffer. Temperature and pH were chosen accordingto growth conditions, as described previously (Kärgel et al.,1996; Zimmer et al., 1997). Cells were washed with PBS, and then1% sodium metaperiodate was added for 1 h to prepare the cellwall for the penetration of the cryoprotectant. The hydrated specimenswere immersed in a cryoprotectant mixture of 25% polyvinyl-pyrrolidone(PVP, K15/MW 10000; Fluka, Buchs, Switzerland) and 1.6 M sucrose,as described in Tokuyasu (1989). To reach complete immersion ofthe cryoprotectant, incubation at 30°C for 2-3 h was strictlynecessary. The cells were subsequently mounted on specimen holders,frozen in liquid nitrogen, and sectioned at $-$ 115°C with an ultracryotomUltracut S attached with a FCS unit (Leica, Heerbrugg, Switzerland).Ultra-thin, thawed cryosections were prepared with glass knifesand placed on formvar/carbon-coated copper grids (200 mesh,hexagonal).

Labeling with primary antibodies and immunogold-complexes (12 nm) was performed according to Griffiths (1993). Finally, thefrozen-thawed sections were stained and stabilized using a mixtureof freshly prepared 3% tungstosilicic acid hydrate (STA; Fluka)and 2.5% polyvinylalcohol (M_r 10,000; Sigma, Deisenhofen,Germany).

CPY* Secretion

Cells were grown to late log phase and then sedimented by centrifugation at 500 × g for 5 min. Cells were washed once withice-cold water and centrifuged again, and the supernatants fromboth centrifugation steps were combined. Proteins were precipitatedwith trichloroacetic acid (10%) for 30 min on ice and sedimentedfor 15 min at 12,000 × g. The pellet was washed twice with ice-coldacetone and dissolved in 100 µl urea buffer (5% SDS, 8 M urea,200 mM Tris-HCl, pH 6.8, 0.1 mM EDTA 1.5% dithiothreithol, 0.03%bromophenol blue). To obtain the intracellular fraction of CPY*,an amount of cells corresponding to 2 OD₆₀₀ were alkaline lysed(Hiller et al., 1996), and the samples were subjected to SDS-PAGEand immunodetection as described previously (Knop et al., 1996a).

Cycloheximide Chase

Cells were grown to log phase at 25°C and incubated for 1 h at 37°C. Cycloheximide was added (0.25 mg/ml), and 2 OD of cellswere taken after 0 and 60 min of chase. Cell extracts were preparedby alkaline lysis method (Hiller et al., 1996), and the sampleswere subjected to SDS-PAGE followed by immunodetection (Knop etal., 1996a).

Antisera

Polyclonal anti-CPY and polyclonal anti-PrA sera were described previously (Finger et al., 1993); anti-Emp47p serum was agenerous gift of H. Riezman (Schröder et al., 1995). Monoclonalanti-CPY and anti-PGK sera were purchased from Molecular Probes(Eugene, OR), HRPO-conjugated anti-mouse antibody from Sigma,monoclonal anti-HA antibody from Babco (HA.11; Berkley, CA), andanti-mouse immunogold-complexes (12 nm) from Dianova (Hamburg,Germany).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We analyzed the degradation of CPY* in mutants defective in anterograde transport between the ER and Golgi. We used the mutantalleles sec12-1, sec23-1, ufe1-1, sed5-1, and sec18-1, which blockvesicular transport at restrictive conditions (Stevens et al.,1982; Hardwick and Pelham, 1992; Lewis and Pelham, 1996). Sec12p,the nucleotide-exchange factor, which recruits Sar1p to the ERmembrane (Campbell and Schekman, 1997), and Sec23p (Kuehn et al.,1998; Springer and Schekman, 1998) are both necessary for COPII-coatedvesicle formation. Ufe1p (Lewis et al., 1997; Patel et al., 1998)and Sed5p (Banfield et al., 1995; Wooding and Pelham, 1998; Tsuiand Banfield, 2000) are t-SNAREs of the ER and Golgi, respectively.They are involved in the fusion of vesicles with the target membrane.Sec18p, the yeast homologue of the mammalian NSF, is requiredfor vesicular transport in multiple stages of the secretory pathway(Graham and Emr, 1991; Mayer et al., 1996). A defect in any ofthese proteins leads to a considerably reduced degradation rateof CPY* (Figure 1, A and B). The half-life of CPY* increases ~2-(sec12-1, sec23-1, and sed5-1) to 6- (ufe1-1) fold in mutant cellscompared with wild type. We had previously analyzed the functionof Sec18p in the degradation of CPY* and PrA*, a rapidly degradedmutant form of proteinase yscA (Finger et al., 1993). Becausethe data had not been quantified, we had concluded that both misfoldedproteins were degraded under restrictive conditions in sec18-1cells. Reinvestigation and quantification of CPY* degradationin these sec18-1 mutant cells, however, revealed a 6- to 7-foldincrease in the half-life of CPY* (Figure 1B). The block of anterogradetransport between ER and Golgi was confirmed by monitoring thematuration of proteinase yscA (PrA) in the mutant strains at restrictiveconditions. In case of the ufe1-1 strain, a tiny fraction of maturedPrA was visible after 60 min of chase; all the other mutants retainedPrA in the proform (Figure 1, C and D). The degradation of CPY*observed in the sec12-1 mutant cells might be due to the actionof a close homologue, Sed4p, which is also involved in the generationof COPII-coated vesicles at the ER membrane (Gimeno et al., 1995).We tested if a deletion of SED4 influences the degradation rateof CPY*, either as a single knockout or in conjunction with thesec12-1 mutation. In both cases there was no detectable changein the half-life of CPY* (our unpublished results).

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Figure 1. CPY* degradation is impaired in mutants defective in ER-to-Golgi transport. Pulse-chase analysis was performed to measure CPY* degradation and maturation of PrA in wild-type and isogenic mutant strains. Cells were shifted to restrictive temperature 5 min before the chase and lysed at the indicated time points. CPY* or PrA were immunoprecipitated and separated by SDS-PAGE. Quantification was done using a PhosphorImager. (A) Formation of COPII-coated vesicles (Sec23p) and ER and Golgi t-SNARES (Ufe1p and Sed 5p) are necessary for efficient degradation of CPY*. (B) CPY* degradation requires a functional Sar1p activating factor (Sec12p) and yeast NSF (Sec18p). (C and D) Transport is blocked in the mutant strains as evidenced by the maturation defect of PrA (pPrA, p1 PrA precursor of the ER; mPrA, mature PrA of the vacuole).

Ufe1p is known to function in two different membrane fusion events: it is involved in the homotypic fusion of ER membranesand in the heterotypic fusion of COPI-coated vesicles with theER membrane. To distinguish between the two different fusion events,we overexpressed the AAA-ATPases Cdc48p and Sec18p in temperature-sensitiveufe1-1 mutant cells. CDC48p is involved in homotypic membranefusion, whereas Sec18p is the homologue used in heterotypic fusionof COPI vesicles with the ER membrane (Lewis et al., 1997; Patelet al., 1998). Overexpression of Cdc48p rescued the temperaturesensitivity of the ufe1-1 mutant (Patel et al., 1998) but wasunable to enhance the degradation of CPY* (our unpublished results).Overexpression of Sec18p, on the other hand, did not rescue thetemperature sensitivity of the ufe1-1 mutant (our unpublishedresults) but, interestingly, was able to partially overcome theufe1-1-mediated degradation defect of CPY* in cells under restrictiveconditions (Figure 2A).

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Figure 2. (A) Over expression of Sec18p partially suppresses the CPY* degradation defect of ufe1-1 mutant cells. Vector (pRS426) or SEC18 on a high copy plasmid (pWO152) were transformed into wild-type (WT) and ufe1-1 mutant cells. Pulse-chase analysis was done as described in Figure 1. (B and C) Synergistic effect of ER-Golgi transport mutants and the unfolded protein response on degradation of CPY*. Pulse-chase analysis was done as described in Figure 1.

As a control, we tested if Sec1p, a protein involved in docking of secretory transport vesicles to the plasma membrane (Novickand Schekman, 1979; Aalto et al., 1997), is involved in ER degradation.As expected, a temperature-sensitive mutant, sec1-1, did not alterthe degradation of CPY* under restrictive conditions comparedwith wild type (our unpublished results). This rules out any unspecificinfluence of defects connected to various sec mutant alleles onER degradation (Mizuta and Warner, 1994).

Using the DNA microarray technique, Travers and coworkers could show that transcription of many genes involved in ER-Golgitransport is upregulated upon stress in the ER. Transcriptionof Sec23p is enhanced by induction of the UPR, whereas transcriptionof Ufe1p is not (Travers et al., 2000). Previous studies did notfind an alteration in CPY* degradation in $Delta$ ire1 cells under nonstressconditions at 30°C (Friedländer et al., 2000). However, we observedthat the degradation rate of CPY* is prolonged in $Delta$ ire1 cellsat 37°C. To examine whether there is a synergistic effect betweenUPR and ER-Golgi transport, we combined the $Delta$ ire1 mutation withmutations in Sec23p and Ufe1p. Indeed, double mutants of $Delta$ ire1with either ufe1-1 or sec23-1 resulted in nearly complete arrestof CPY* degradation under restrictive conditions (Figure 2, BandC).

Consequently, we tested if a block in retrograde transport from the Golgi to the ER would influence the degradation rate ofCPY* as much as a block in anterograde transport does. We measuredthe degradation of CPY* in yeast cells defective in Sec21p orSec27p, two components of the COPI complex (Hosobuchi et al.,1992; Duden et al., 1994; Letourneur et al., 1994). As shown inFigure 3, A and B, degradation of CPY* is only moderately affectedin sec21-1 or sec27-1 cells at restrictive conditions. It is knownthat proteins, which cannot be retrograde transported from theGolgi to the ER, may travel to the vacuole for degradation. Therefore,we combined a mutation in Sec27p with a deletion of the PEP4 gene,leading to a proteolysis defective vacuole (Knop et al., 1993;Van Den Hazel et al., 1996), to check if vacuolar degradationcontributes to the decay of CPY* in this COPI mutant. We foundthat degradation of CPY* was not altered in the double mutant(Figure 3B), whereas a pep4 single mutant degrades CPY* like awild-type strain (our unpublished results and Figure 5B). Anterogradetransport is partially affected in sec21-1 and to a lesser degreein sec27-1 cells (Letourneur et al., 1994). We measured the maturationprocess of PrA, applying the conditions for the CPY* degradationexperiment, and found that in fact PrA is not fully matured inthe mutant cells after 60 min of chase (Figure 3C). In wild-typecells 80% of PrA is matured after 60 min of chase, whereas insec21-1 cells only 64% and in sec27-1 cells 74% is in the matureform. Retrograde transport is defective in these two mutants at37°C. It is known that Emp47p is degraded in the vacuole, whenits recycling via COPI-coated vesicles is inhibited (Lewis andPelham, 1996; Schröder-Köhne et al., 1998). We, therefore, testedthe stability of Emp47p in sec21-1 and sec27-1 cells and foundthat Emp47p is degraded rapidly in the mutants, but it is stablein the respective wild-type cells at restrictive conditions (Figure3D). This shows that even although retrograde transport is defectivein these cells, CPY* is degraded efficiently.

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Figure 3. CPY* degradation is affected only moderately in cells defective in COPI-coated vesicle formation at restrictive temperature. Pulse-chase analysis was performed as described in Figure 1, except that the cells were shifted to restrictive temperature 60 min before the chase. (A) CPY* degradation in isogenic wild-type and sec21-1 mutant strain. (B) CPY* degradation in isogenic wild-type, sec27-1, and sec27-1 $Delta$ pep4 mutant strains. (C) Maturation of PrA was measured in a pulse-chase experiment in COPI mutant and isogenic wild-type strains. The experiment was done as described for Figure 3A, except that the cells were labeled with radioactive methionine for 10 min. (D) COPI-coated vesicle transport is affected in the mutant strains under the conditions used. Emp47p degradation was followed in a cycloheximide chase experiment after a 60-min preincubation at 37°C. Equal amounts of cells were taken at the indicated time points. Pgk1p served as a loading control.

One of the possible models that would explain these results is the existence of a special ER-derived compartment for degradation,as proposed recently for mammalian cells by Kamhi-Nesher et al.(2001). To test this model, we analyzed the localization of CPY*by electron microscopy and immuno-gold visualization of an HA-taggedversion of CPY*. CPY*-HA is degraded in the same way and withsimilar kinetics as nontagged CPY* (our unpublished results).CPY*-HA is localized to the ER/nuclear envelope and to the peripheralER, whereas the later compartments of the secretory pathway arealmost free of label in wild-type cells (Figure 4A). A yeast straindeleted in Der1p, which is defective in the degradation of CPY*(Knop et al., 1996a), was used to analyze whether CPY*-HA is accumulatingin a novel compartment. In $Delta$ der1 cells, as in wild-type, mostof the CPY*-HA was found at the ER/nuclear envelope and the peripheralER. Additionally, CPY*-HA was found in the Golgi apparatus andthe vacuole, and a fraction was secreted outside the cell (Figure4, B and C). This finding complements the results of Knop et al.,1996a, who showed Golgi glycosylation of CPY* in Der1p mutantcells. In control cells, not expressing CPY*-HA, few gold particlescan typically be found inside the nucleus and in the cytosol butnot in any membraneous structures (Figure 4D).

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Figure 4. Localization of CPY*-HA by immuno-EM. Ultra-thin cryosections of wild-type (A) and Der1p-deleted cells (B and C) expressing HA-tagged CPY* or wild-type cells without tag (D) were labeled with antibodies against HA and anti-mouse-gold complexes (12 nm). Yeast strains in A, B, and C were transformed with plasmid pCT52, carrying CPY*-HA under the control of the CUP1 promoter. The expression of CPY*-HA was induced with addition of copper sulfate (100 µM final concentration) for 3 h. (A) CPY*-HA is localized to the ER in wild-type cells. (B) CPY*-HA is distributed in structures of the secretory system in $Delta$ der1 cells. (C) $Delta$ der1 cells secrete CPY*-HA to the outside of the cell. (D) Unspecific staining of the used antibodies in wild-type cells. N, nucleus; M, mitochondrion; V, vacuole; G, Golgi elements. Bars, 500 nm.

The localization of CPY* was also analyzed by Western blotting, which confirmed the EM data: in wild-type cells a minor fractionof CPY* was secreted into the medium, whereas in $Delta$ der1 and $Delta$ der3/hrd1cells more CPY* appeared in the medium (Figure 5A). Additionally,the amount of secreted CPY* was higher than that of Kar2p in thesecells, as evidenced by a very faint Kar2p signal in the extracellularfraction (Figure 5A). It is known that Kar2p is secreted whenthe HDEL retrieval pathway is saturated (Belden and Barlowe, 2001).To analyze the fate of CPY* in the vacuole, we performed pulse-chaseanalysis in cells with impaired vacuolar degradation due to deletionof the PEP4 gene (Knop et al., 1993; Van Den Hazel et al., 1996).In $Delta$ pep4 cells CPY* was degraded as in wild-type cells; however,in $Delta$ der1 $Delta$ pep4 double mutants the degradation was slower thanin $Delta$ der1 single mutants (Figure 5B).

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Figure 5. (A) CPY* is secreted into the medium. Cellular and secreted CPY* was analyzed by SDS-PAGE and immunodetection. The same blot was reprobed against Kar2p. Approximately five times more material was loaded in the extracellular fraction. (B) Vacuolar hydrolysis contributes to degradation of CPY* in $Delta$ der1 cells. Degradation of CPY* was measured by pulse-chase analysis in yeast strains defective in vacuolar hydrolysis ( $Delta$ pep4), ER degradation ( $Delta$ der1), or double mutants ( $Delta$ pep4 $Delta$ der1).

The EM images revealed that in cells deficient in ER degradation some interesting morphological changes are visible. In thesecells ( $Delta$ der1, $Delta$ der3/hrd1, and $Delta$ hrd3) the Golgi apparatus appearsas stacked cisternae in many cells (Figure 6, B and C, and ourunpublished results), whereas a typical wild-type cell containsdisconnected Golgi structures (Figure 6A). Stacked Golgi structureswere previously observed in yeast mutant cells defective in intra-Golgitransport, such as in sec7-1 cells at nonpermissive conditions(Rambourg et al., 1993) but rarely in wild-type cells (Rambourget al., 1995). Mutants defective in ER degradation ( $Delta$ der1, $Delta$ der3/hrd1,and $Delta$ hrd3) also exhibit a considerably proliferated ER (Figure6D and our unpublished results). These morphological changes areabsent in cells where ER degradation is abolished in conjunctionwith the unfolded protein response. In $Delta$ der1 $Delta$ ire1 cells the ERdoes not proliferate and the Golgi apparatus has normal appearance(our unpublished results).

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Figure 6. Morphology of secretory organelles is changed in mutants defective in ER degradation. (A) Wild-type. (B) Golgi structure in $Delta$ der1 cells. (C) Golgi structures present in Der3/Hrd1p-deficient cells. (D) ER proliferates in $Delta$ der3/hrd1 cells. N, nucleus; M, mitochondrion; V, vacuole; ER, endoplasmic reticulum. Bars, 1000 and 500 nm, respectively.

These observations raised the question of whether the morphological changes in the ER and Golgi influence the secretory functionof these organelles. To address this question, we measured thematuration kinetics of wild-type CPY in wild-type and $Delta$ der1 mutantcells. Distinct forms of CPY reflect the transport of this enzymefrom the ER via the Golgi to the vacuole. The core glycosylatedpro-CPY precursor in the ER has a molecular mass of ~67 kDa (p1CPY).In the Golgi, the carbohydrate of CPY is modified, resulting inthe p2CPY form of 69 kDa. After transport to the vacuole, CPYis matured (mCPY) to a final form of 61 kDa (Rendueles and Wolf,1988). Figure 7, A and B, shows that the transport of wild-typeCPY is not delayed to a significant degree in cells lacking Der1p.The calculated ratio between Golgi p2CPY and vacuolar mCPY speciesis almost the same in wild-type and $Delta$ der1 mutant cells at thedifferent time points (Figure 7B). However, when CPY*-HA is expressedsimultaneously with wild-type CPY in Der1p-deficient cells, thematuration of CPY from the p2CPY Golgi form to the mature vacuolarform is considerably delayed (Figure 7C). The ratio between p2and mCPY is higher in $Delta$ der1 than in wild-type cells when CPY*-HAis coexpressed, indicating a slower transport of the p2CPY form(Figure 7D). Surprisingly, the exit of pro-CPY from the ER seemsto be undisturbed: there is no difference in the rate of disappearanceof p1CPY between wild-type and $Delta$ der1 cells expressing CPY*-HA(Figure 7F), and it is also the same as that observed in wild-typecells not coexpressing CPY or CPY*-HA (our unpublished results).As a control, we expressed CPY exogenously in wild-type and $Delta$ der1cells and followed the maturation of CPY. Under these conditions,every step of the process was delayed in both strains, startingwith a slower exit from the ER (Figure 7, E and F). Taken together,the EM data and the CPY maturation experiments suggest that escapeof unfolded proteins from the ER disturbs the secretory competenceof the later stages of the secretory pathway.

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Figure 7. Maturation of CPY is prolonged, upon presence of unfolded proteins in the secretory pathway. Cells expressing CPY were labeled for 5 min with radioactive methionine. Cells were lysed at the indicated time points and treated as described in Figure 1. The positions of p1 (ER), p2 (Golgi), m (vacuolar) CPY and CPY*-HA are shown. (A) Maturation of CPY is not dependent on the presence of Der1p. (B) Calculated ratio between p2 and mCPY in wild-type and $Delta$ der1 cells. (C) Expression of CPY*-HA leads to delay in maturation of CPY in $Delta$ der1 cells. Plasmid pCT43, carrying CPY*-HA under the control of the TDH3 promoter, was introduced into wild-type and $Delta$ der1 cells. (D) Calculated ratio between p2 and mCPY in wild-type and $Delta$ der1 cells expressing additional CPY*-HA. (E) Expression of additional CPY from the TDH3 promoter leads to delayed maturation of CPY in wild-type and $Delta$ der1 cells. (F) Conversion of the p1-form to the p2 Golgi form of CPY in wild-type and $Delta$ der1 cells expressing additional CPY or CPY*-HA, respectively.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Using mutants defective in ER-to-Golgi traffic, we discovered a connection between the secretory competence of the ER itselfand the degradation of the ERAD substrate CPY*. Mutants defectivein Ufe1p, Sec12p, Sec23p, Sed5p, and Sec18p exhibited an extendedhalf-life of CPY* (Figure 1). After completion of our studies,reports appeared that also communicate disturbed degradation ofsoluble ER degradation substrates in mutants defective in ER-Golgitransport (Caldwell et al., 2001; Vashist et al., 2001). The authorsgive two explanations for the involvement of ER-to-Golgi transportin ER degradation: (i) Soluble ER substrates may travel to theGolgi and back to the ER, either to receive a modification thatenhances degradation (Caldwell et al., 2001) or as the defaultroute to degradation (Vashist et al., 2001). (ii) Alternatively,an yet unidentified factor, which is required for the degradationof soluble substrates, cycles between ER and Golgi. In this model,the substrate itself remains in the ER (Caldwell et al., 2001).

Our results lead to different conclusions: in the sec12-1, sec18-1, and sec23-1 mutants, ER-to-Golgi transport is blockedcompletely as evidenced by the lack of the Golgi localized p2CPYspecies (Stevens et al., 1982) or by the maturation defect ofPrA (Figure 1, C and D). In contrast, degradation of CPY* is notcompletely blocked in these mutants (Figure 1, A and B). Instead,degradation of CPY* takes place at different rates in the variousER-Golgi trafficking mutants tested; the delay in degradationranges between a factor of 2 (sec12-1, sec23-1, and sed5-1 mutantstrains) and 6-7 (sec18-1 and ufe1-1 mutants). Deletion of Sed4p,a close homologue of Sec12p, in the presence of the sec12-1 mutation,did not enhance the half-life of CPY*. Because ER-to-Golgi trafficis blocked in these mutants, it is hard to envisage how some CPY*could still reach the Golgi to receive a specific modificationor why the degradation route would be changed in sec12-1, sec23-1,or sed5-1 but not in sec18-1 or ufe1-1 cells. In COPI mutant cells(sec21-1 and sec27-1), only a moderate alteration in the degradationof CPY* compared with wild-type is visible (Figure 3, A and B),despite the fact that retrograde traffic from the Golgi to theER is defective (Figure 3D and Letourneur et al., 1994). If CPY*would travel to the Golgi and back to the ER before degradation,one would expect a much larger influence of COPI-coat mutantson degradation of CPY*. Because the half-life of CPY* is not increasedin sec27-1 $Delta$ pep4 double-mutant cells, we conclude that the vacuoledoes not contribute to the degradation seen in sec27-1 cells (Figure3B). All together, the transport defects of the various mutantscannot be correlated with the degradation pattern of CPY*. Thesefindings, therefore, argue against the idea of a relocation ofCPY* to the Golgi and then back to the ER or of the recyclingof a proteinaceous factor between these compartments for efficientdegradation of CPY*. Only a yet-unknown Golgi-ER retrieval mechanismcould possibly apply for a cycling-dependent degradation mechanism.Another recent publication reports that mutations in the earlysecretory pathway severely affect the structure of the ER (Prinzet al., 2000). They show that ufe1-1 or sec23-1 mutant cells,two mutants also used in our studies, exhibit a dramatically reducedamount of peripheral ER and a considerably disorganized organelleat nonpermissive temperature (Prinz et al., 2000). We find thatunder the same conditions degradation of CPY* is prolonged inthese mutants (Figure 1A). Another possible explanation is thatthe mislocalization of Kar2p observed in various ER-Golgi transportmutants (Nishikawa et al., 1994) leads to defective degradation.Kar2p is necessary for degradation of CPY* (Plemper et al., 1997)but is not involved in the degradation of membrane proteins (Plemperet al., 1998; Kiser et al., 2001; Zhang et al., 2001). This modelwould explain why misfolded membrane proteins are degraded efficientlyin the ER-Golgi transport mutants (Biederer et al., 1996; Katzmannet al., 1999; Vashist et al., 2001), whereas CPY* is not. Takentogether, we conclude that the morphological disturbance of theER, mislocalization of Kar2p, or both, are the cause of the changesin CPY* degradation. Analysis of the localization of HA-taggedCPY* via immuno-gold EM revealed that the protein resides at theER/nuclear envelope and the peripheral ER. These EM images donot indicate the existence of a novel compartment, specializedin ER degradation (Figure 4, A-C), as recently proposed for mammaliancells (Kamhi-Nesher et al., 2001). In the light of the EM data,the degradation behavior of CPY* in the ER-Golgi transport mutantsas well as the data of Prinz et al. (2000) and Nishikawa et al.(1994), we suggest that the decrease in degradation of CPY* isdue to indirect or secondary effects caused by the mutations thatlead to impaired ER-Golgi transport. The severe alteration inCPY* degradation observed in double mutants defective in Sec23por Ufe1p and UPR signaling due to deletion of Ire1p (Figure 2,B and C), can be explained similarly: the amount of ER is diminished,chaperones like Kar2p are mislocalized, and the possibility toincrease expression of proteins involved in ER-stress relieveis abolished. Recovery of CPY* degradation upon overexpressionof Sec18p in ufe1-1 mutants indicates that the involvement ofUfe1p in vesicular transport is necessary to maintain proper CPY*degradation and that this is independent of its involvement inhomotypic membrane fusion exerted together with Cdc48p (Figure2A). Recent studies show that Cdc48p does indeed take part inCPY* degradation, being involved in retro-translocation of themalfolded protein into the cytosol (Ye et al., 2001; Bays et al.,2001b; Rabinovitch et al., 2002; Jarosch et al., 2002).

The ER is considerably enlarged in $Delta$ der1, $Delta$ der3/hrd1, and $Delta$ hrd3 cells (Figure 6D and our unpublished results). This alterationis most likely controlled by the UPR, because many genes involvedin lipid metabolism are also upregulated upon ER stress (Traverset al., 2000). As expected, a $Delta$ der1 $Delta$ ire1 double knockout strainhas no proliferated ER (our unpublished results). The appearanceof Golgi stacks could indicate a defect in intra-Golgi transportin the mutants deficient in ER degradation, which is less severethan the one seen in the sec7-1 mutant at restrictive conditionsbut significant enough to change the morphology of the organelle.On disruption of CPY* degradation by deletion of Der1p, we findsome CPY*-HA in the Golgi apparatus, in the vacuole and in secretedform (Figure 4, B and C). This indicates a "leakage" of CPY*-HAout of the ER under these conditions. In addition, in a straindeleted for Der1p and Pep4p, CPY* has a longer half-life thanin a strain lacking only Der1p, indicating transport of a fractionof CPY* into the vacuole. This finding complements the observationof Knop et al. (1996a), who reported some Golgi glycosylationof CPY* in $Delta$ der1 cells. Soluble, misfolded proteins can escapefrom the ER when their degradation is abolished. The reason isprobably the saturation of the retrieval pathway from the Golgiback to the ER when too many unfolded proteins are present inthe ER. It is known that the HDEL receptor takes part in the retentionof unfolded proteins in the ER by recycling them back from theGolgi (Knop et al., 1996a; Yamamoto et al., 2001). Unfolded proteinsthat escape the retention machinery travel along the secretorypathway to the vacuole or are secreted (Figures 4, B and C, and5). This seems to disturb the secretory pathway in a yet unknownway, as delivery of wild-type CPY from the Golgi to the vacuoleis delayed in $Delta$ der1 cells simultaneously expressing malfoldedCPY*-HA (Figure 7). This delay can be explained by a defect intransport through the Golgi due to the presence of misfolded proteinsor, alternatively, by a competition between CPY and CPY*-HA forthe CPY sorting receptor, Vps10p (Stack et al., 1995). Perturbationsin vacuolar function may also explain this phenomenon. The maturationdefect observed in $Delta$ der1 cells coexpressing CPY*-HA is not simplya consequence of overloading in the secretory pathway. Overloadingthrough expression of additional CPY results in slower transportin every step of the secretory pathway, e.g., the half-life inexit from the ER is roughly doubled (Figure 7F). In $Delta$ der1 cellsexpressing CPY*-HA only the later transport or maturation stepsare affected, which seems to be a consequence of unfolded proteinspresent in the secretory pathway (Figure 7, C and D). The datapresented here indicate that efficient ER degradation requiresan ER fully competent in secretion and, vice versa, that efficientsecretion depends on an undisturbed quality control machineryin theER.

	ACKNOWLEDGMENTS

The authors thank M. Vogel for the preparation of the cryosections, R. Hitt, J. Strayle, H. Rudolph, H. Pelham, T. Sommer,H. Riezman, and C. Barlowe for antibodies, plasmids, and strains.We are grateful to Z. Kostova, R. Hitt, J. Strayle, S. Jäger,and the members of the Sommer lab for helpful discussions andElisabeth Tosta for help with the manuscript. This work was supportedby the Deutsche Forschungsgemeinschaft, Bonn; the German-IsraeliProject Cooperation (DIP) of the Bundesministerium für Bildungund Forschung (BMBF); and the Fonds der Chemischen Industrie,Frankfurt.

	FOOTNOTES

Corresponding author. E-mail address: dieter.wolf{at}po.uni-stuttgart.de.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.01-08-0399. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.01-08-0399.

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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				Z. Kostova, J. Mariano, S. Scholz, C. Koenig, and A. M. Weissman A Ubc7p-binding domain in Cue1p activates ER-associated protein degradation J. Cell Sci., May 1, 2009; 122(9): 1374 - 1381. [Abstract] [Full Text] [PDF]

				S. Kohlmann, A. Schafer, and D. H. Wolf Ubiquitin Ligase Hul5 Is Required for Fragment-specific Substrate Degradation in Endoplasmic Reticulum-associated Degradation J. Biol. Chem., June 13, 2008; 283(24): 16374 - 16383. [Abstract] [Full Text] [PDF]

				J. J. Caramelo and A. J. Parodi Getting In and Out from Calnexin/Calreticulin Cycles J. Biol. Chem., April 18, 2008; 283(16): 10221 - 10225. [Full Text] [PDF]

				H. Hirayama, M. Fujita, T. Yoko-o, and Y. Jigami *O-Mannosylation is Required for Degradation of the Endoplasmic Reticulum-associated Degradation Substrate Gas1p via the Ubiquitin/Proteasome Pathway in Saccharomyces cerevisiae** J. Biochem., April 1, 2008; 143(4): 555 - 567. [Abstract] [Full Text] [PDF]

				N. Mimura, S. Yuasa, M. Soma, H. Jin, K. Kimura, S. Goto, H. Koseki, and T. Aoe Altered Quality Control in the Endoplasmic Reticulum Causes Cortical Dysplasia in Knock-In Mice Expressing a Mutant BiP Mol. Cell. Biol., January 1, 2008; 28(1): 293 - 301. [Abstract] [Full Text] [PDF]

				T. Kato, K. Kitamura, M. Maeda, Y. Kimura, T. Katayama, H. Ashida, and K. Yamamoto Free Oligosaccharides in the Cytosol of Caenorhabditis elegans Are Generated through Endoplasmic Reticulum-Golgi Trafficking J. Biol. Chem., July 27, 2007; 282(30): 22080 - 22088. [Abstract] [Full Text] [PDF]

				M. M. Kincaid and A. A. Cooper Misfolded Proteins Traffic from the Endoplasmic Reticulum (ER) Due to ER Export Signals Mol. Biol. Cell, February 1, 2007; 18(2): 455 - 463. [Abstract] [Full Text] [PDF]

				G. H.-F. Yam, K. Gaplovska-Kysela, C. Zuber, and J. Roth Aggregated Myocilin Induces Russell Bodies and Causes Apoptosis: Implications for the Pathogenesis of Myocilin-Caused Primary Open-Angle Glaucoma Am. J. Pathol., January 1, 2007; 170(1): 100 - 109. [Abstract] [Full Text] [PDF]

				N. Hiramatsu, A. Kasai, K. Hayakawa, J. Yao, and M. Kitamura Real-time detection and continuous monitoring of ER stress in vitro and in vivo by ES-TRAP: evidence for systemic, transient ER stress during endotoxemia Nucleic Acids Res., July 28, 2006; 34(13): e93 - e93. [Abstract] [Full Text] [PDF]

				C. Appenzeller-Herzog and H.-P. Hauri The ER-Golgi intermediate compartment (ERGIC): in search of its identity and function J. Cell Sci., June 1, 2006; 119(11): 2173 - 2183. [Abstract] [Full Text] [PDF]

				P. Pimpl, J. P. Taylor, C. Snowden, S. Hillmer, D. G. Robinson, and J. Denecke Golgi-Mediated Vacuolar Sorting of the Endoplasmic Reticulum Chaperone BiP May Play an Active Role in Quality Control within the Secretory Pathway PLANT CELL, January 1, 2006; 18(1): 198 - 211. [Abstract] [Full Text] [PDF]

				K. B. Kruse, J. L. Brodsky, and A. A. McCracken Characterization of an ERAD Gene as VPS30/ATG6 Reveals Two Alternative and Functionally Distinct Protein Quality Control Pathways: One for Soluble Z Variant of Human {alpha}-1 Proteinase Inhibitor (A1PiZ) and Another for Aggregates of A1PiZ Mol. Biol. Cell, January 1, 2006; 17(1): 203 - 212. [Abstract] [Full Text] [PDF]

				C. Castro-Fernandez, G. Maya-Nunez, and P. M. Conn Beyond the Signal Sequence: Protein Routing in Health and Disease Endocr. Rev., June 1, 2005; 26(4): 479 - 503. [Abstract] [Full Text] [PDF]

				S.-i. Nishikawa, J. L. Brodsky, and K. Nakatsukasa Roles of Molecular Chaperones in Endoplasmic Reticulum (ER) Quality Control and ER-Associated Degradation (ERAD) J. Biochem., May 1, 2005; 137(5): 551 - 555. [Abstract] [Full Text] [PDF]

				M. E. Kirst, D. J. Meyer, B. C. Gibbon, R. Jung, and R. S. Boston Identification and Characterization of Endoplasmic Reticulum-Associated Degradation Proteins Differentially Affected by Endoplasmic Reticulum Stress Plant Physiology, May 1, 2005; 138(1): 218 - 231. [Abstract] [Full Text] [PDF]

				Z. Kostova and D. H. Wolf Importance of carbohydrate positioning in the recognition of mutated CPY for ER-associated degradation J. Cell Sci., April 1, 2005; 118(7): 1485 - 1492. [Abstract] [Full Text] [PDF]

				J. Ramos-Castaneda, Y.-n. Park, M. Liu, K. Hauser, H. Rudolph, G. E. Shull, M. F. Jonkman, K. Mori, S. Ikeda, H. Ogawa, et al. Deficiency of ATP2C1, a Golgi Ion Pump, Induces Secretory Pathway Defects in Endoplasmic Reticulum (ER)-associated Degradation and Sensitivity to ER Stress J. Biol. Chem., March 11, 2005; 280(10): 9467 - 9473. [Abstract] [Full Text] [PDF]

				H. Hamada, M. Suzuki, S. Yuasa, N. Mimura, N. Shinozuka, Y. Takada, M. Suzuki, T. Nishino, H. Nakaya, H. Koseki, et al. Dilated Cardiomyopathy Caused by Aberrant Endoplasmic Reticulum Quality Control in Mutant KDEL Receptor Transgenic Mice Mol. Cell. Biol., September 15, 2004; 24(18): 8007 - 8017. [Abstract] [Full Text] [PDF]

				G. Huyer, W. F. Piluek, Z. Fansler, S. G. Kreft, M. Hochstrasser, J. L. Brodsky, and S. Michaelis Distinct Machinery Is Required in Saccharomyces cerevisiae for the Endoplasmic Reticulum-associated Degradation of a Multispanning Membrane Protein and a Soluble Luminal Protein J. Biol. Chem., September 10, 2004; 279(37): 38369 - 38378. [Abstract] [Full Text] [PDF]

				L. M. Sevilla, S. S. Comstock, K. Swier, and J. Miller Endoplasmic Reticulum-Associated Degradation-Induced Dissociation of Class II Invariant Chain Complexes Containing a Glycosylation-Deficient Form of p41 J. Immunol., August 15, 2004; 173(4): 2586 - 2593. [Abstract] [Full Text] [PDF]

				S. Nadanaka, H. Yoshida, F. Kano, M. Murata, and K. Mori Activation of Mammalian Unfolded Protein Response Is Compatible with the Quality Control System Operating in the Endoplasmic Reticulum Mol. Biol. Cell, June 1, 2004; 15(6): 2537 - 2548. [Abstract] [Full Text] [PDF]

				C. M. Coughlan, J. L. Walker, J. C. Cochran, K. D. Wittrup, and J. L. Brodsky Degradation of Mutated Bovine Pancreatic Trypsin Inhibitor in the Yeast Vacuole Suggests Post-endoplasmic Reticulum Protein Quality Control J. Biol. Chem., April 9, 2004; 279(15): 15289 - 15297. [Abstract] [Full Text] [PDF]

				M. M. Khan, T. Nomura, T. Chiba, K. Tanaka, H. Yoshida, K. Mori, and S. Ishii The Fusion Oncoprotein PML-RAR{alpha} Induces Endoplasmic Reticulum (ER)-associated Degradation of N-CoR and ER Stress J. Biol. Chem., March 19, 2004; 279(12): 11814 - 11824. [Abstract] [Full Text] [PDF]

				C. Taxis, R. Hitt, S.-H. Park, P. M. Deak, Z. Kostova, and D. H. Wolf Use of Modular Substrates Demonstrates Mechanistic Diversity and Reveals Differences in Chaperone Requirement of ERAD J. Biol. Chem., September 19, 2003; 278(38): 35903 - 35913. [Abstract] [Full Text] [PDF]

				K. Yamamoto, H. Hamada, H. Shinkai, Y. Kohno, H. Koseki, and T. Aoe The KDEL Receptor Modulates the Endoplasmic Reticulum Stress Response through Mitogen-activated Protein Kinase Signaling Cascades J. Biol. Chem., September 5, 2003; 278(36): 34525 - 34532. [Abstract] [Full Text] [PDF]

				L. Fu and E. Sztul Traffic-independent function of the Sar1p/COPII machinery in proteasomal sorting of the cystic fibrosis transmembrane conductance regulator J. Cell Biol., January 21, 2003; 160(2): 157 - 163. [Abstract] [Full Text] [PDF]