Ceramide Accumulation Uncovers a Cycling Pathway for the cis-Golgi Network Marker, Infectious Bronchitis Virus M Protein

doi:10.1083/jcb.139.6.1411

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© The Rockefeller University Press, 0021-9525/1997//1411 $5.00
The Journal of Cell Biology, Volume 139, Number 6, , 1997 1411-1418

Article

Ceramide Accumulation Uncovers a Cycling Pathway for the cis-Golgi Network Marker, Infectious Bronchitis Virus M Protein

Michael Maceyka and Carolyn E. Machamer

Department of Cell Biology and Anatomy, The Johns Hopkins School of Medicine, Baltimore, Maryland 21205

The M glycoprotein from the avian coronavirus, infectious bronchitisvirus (IBV), contains information for localization to the cis-Golginetwork in its first transmembrane domain. We hypothesize thatlocalization to the Golgi complex may depend in part on specificinteractions between protein transmembrane domains and membranelipids. Because the site of sphingolipid synthesis overlapsthe localization of IBV M, we asked whether perturbation ofsphingolipids affected localization of IBV M. Short-term treatment with two inhibitors of sphingolipid synthesis had no effecton localization of IBV M or other Golgi markers. Thus, ongoingsynthesis of these lipids was not required for proper localization.Surprisingly, a third inhibitor, d,l-threo-1-phenyl-2-decanoylamino-3-morpholino-1-propanol (PDMP), shifted the steady-state distribution ofIBV M from the Golgi complex to the ER. This effect was rapidand reversible and was also observed for ERGIC-53 but not forGolgi stack proteins. At the concentration of PDMP used, conversionof ceramide into both glucosylceramide and sphingomyelin wasinhibited. Pretreatment with upstream inhibitors partially reversed the effects of PDMP, suggesting that ceramide accumulationmediates the PDMP-induced alterations. Indeed, an increasein cellular ceramide was measured in PDMP-treated cells. Wepropose that IBV M is at least in part localized by retrievalmechanisms. Further, ceramide accumulation reveals this cycleby upsetting the balance of anterograde and retrograde trafficand/ or disrupting retention by altering bilayer dynamics.

Abbreviations used in this paper: CGN, cis-Golgi network; GlcCer, glucosylceramide; IBV, infectious bronchitis virus; IC, intermediate compartment; PDMP, d,l-threo-1-phenyl-2-decanoylamino-3-morpholino-1-propanol; SM, sphingomyelin; VSV, vesicular stomatitis virus.

THE organelles of the classical secretory pathway must maintaintheir identity despite a large flux of lipids and proteins.Two models have emerged to explain how proteins can be maintainedin specific compartments (Machamer, 1993; Nilsson and Warren, 1994). The retention model proposes that proteins are efficiently anchored in the appropriate compartment. The retrieval modelproposes that proteins are continually recycled from latercompartments. The two models are not mutually exclusive; indeedmost proteins within the secretory pathway probably use bothmechanisms for localization, albeit to differing extents. Anexample of this is the localization of the ER resident proteinBiP, which contains a KDEL retrieval signal but is only slowlysecreted when this signal is removed (Munro and Pelham, 1987).This suggests that other parts of the molecule may containretention information.

The M glycoprotein from the avian coronavirus, infectious bronchitisvirus (IBV),¹ is a model protein for studying localization tothe early secretory pathway. Immunoelectron microscopy showedthat IBV M expressed in the absence of other IBV proteins wasfound in the tubulo- vesicular structures at the entry or cisface of the Golgi stack, as well as the first or second cisternaof the Golgi stack (Machamer et al., 1990; Sodeik et al., 1993).We will refer to this region as the cis-Golgi network (CGN;Mellman and Simons, 1992). Defined in this way, we would considerthe CGN to at least partially overlap with the intermediatecompartment (IC), defined by such markers as ERGIC-53 or p58(Schweizer et al., 1988; Lahtinen et al., 1996). The firsttransmembrane domain of IBV M is sufficient to target chimericproteins to the CGN (Swift and Machamer, 1991; Machamer et al., 1993).Although the transmembrane domains of other Golgi proteinsalso contain targeting information, no consensus motif for localizationhas been identified (for review see Colley, 1997). We are intriguedby the possibility that the targeting of Golgi membrane proteinsmay in part depend on interactions between their transmembranedomains and specific membrane lipids.

Independent studies demonstrate that the lipid compositionsof membranes differ at each stage of the secretory pathway(Keenan and Morre, 1970; Cluett et al., 1997; for review seevan Meer, 1993). Sphingolipids, including sphingomyelin (SM)and glucosylceramide (GlcCer), the precursor to all gangliosides,are one class of lipids thought to increase in relative concentrationthrough the secretory pathway. Ceramide, the precursor of sphingolipids,is synthesized in the ER. In rat liver, ceramide is convertedinto the different classes of sphingolipids by enzymes localized to the CGN and the cis- and medial-Golgi cisternae (Futerman et al., 1990;Futerman and Pagano, 1991). When expressed from a recombinantvaccinia virus, IBV M is localized to the CGN in several celltypes, and its localization presumably overlaps with that ofSM and GlcCer synthase activities. This led us to speculatethat there may be a link between sphingolipid synthesis andthe localization of IBV M. To address this question we testedthe effects of three sphingolipid synthesis inhibitors on thesteady-state localization of IBV M. We observed a dramaticredistribution of IBV M induced by one of these inhibitors,the glucosylceramide analogue d,l-threo-1-phenyl-2-decanoylamino-3-morpholino-1-propanol (PDMP). Use of upstream inhibitors coupledwith lipid analysis suggested that the PDMP effects are mediatedby the accumulation of the precursor ceramide. Because IBVM can be induced to move to the ER, we propose that IBV M isat least in part localized by retrieval mechanisms.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Materials
FCS was from Atlanta Biologicals (Norcross, GA); fumonisin B1was from Calbiochem (La Jolla, CA); chromatography plates werefrom E. Merck (Darmstadt, Germany); endoglycosidase H (endoH) from New England Biolabs (Beverly, MA); N-hexanoylsphingosine(C₆Cer), lipid standards, and PDMP were from Matreya (PleasantGap, PA); [³H]palmitate (50 Ci/mmol) was from DuPont-NEN (Wilmington,DE); Pro-Mix (>1,000 mCi/mmol [³⁵S]methionine) was fromAmersham Intl. (Arlington Heights, IL); DME, tissue culture–gradetrypsin, and penicillin-streptomycin were from GIBCO BRL (Gaithersburg,MD); all other reagents were from Sigma Chemical Co. (St. Louis,MO).

Antibodies were obtained as follows: monoclonal anti-Bip, Stressgen (Victoria, BC, Canada); monoclonal anti-giantin and monoclonalanti-ERGIC-53, Hans-Peter Hauri (Basel, Switzerland); polyclonalanti–β-COP, Jennifer Lippincott-Schwartz (NationalInstitutes of Health, Bethesda, MD); polyclonal ${alpha}$ -mannosidaseII, Marilyn Farquhar (University of California at San Diego,La Jolla, CA) and Kelley Moreman (University of Georgia, Athens,GA); polyclonal antibodies to IBV M and vesicular stomatitisvirus (VSV) were prepared as described (Machamer and Rose, 1987; Weisz et al., 1993, respectively); Texas red– and FITC-conjugatedsecondary antibodies, Jackson ImmunoResearch (West Grove, PA).

Methods
Cell Culture.
Tissue culture cells were grown in DME supplemented with 5%(BHK-21) or 10% (Vero) FCS. Cells were grown at 37°C inan atmosphere of 5% CO₂.

Pulse–Chase Labeling.
Pulse–chase experiments were performed as previouslydescribed (Rosenwald et al., 1992; Weisz et al., 1993). Briefly, cells were plated in 35-mm dishes the night before the experimentto be 90% confluent the next day. VSV (San Juan strain, Indianaserotype) was adsorbed for 30 min in 0.5 ml of serum-free DME.At 4 h after infection, the cells were starved for methioninefor 15 min. Cells were then pulsed for 5 min with 50 µCi³⁵S-Pro-mix and chased for the indicated amount of time inthe presence or absence of the indicated drugs. The isopropanol carrier alone had no effect on the rate of transport of VSVG protein. After the chase, cells were washed once with coldPBS and lysed in detergent. VSV G protein was then immunoprecipitated,treated with endo H as described (Rosenwald et al., 1992),separated by SDS-PAGE, and visualized by fluorography. EndoH–sensitive and -resistant forms of the VSV G proteinwere quantitated by densitometry.

Indirect Immunofluorescence Microscopy.
These experiments were performed as previously described (Swift and Machamer, 1991).Briefly, cells were infected for 30 min with a recombinantvaccinia virus encoding IBV M, and the indicated treatmentswere begun 4 h after infection. For experiments using exogenousceramides, the soluble short-chain analogues of ceramide wereadded to cells as a complex with 0.34 mg/ml defatted BSA asdescribed (Pagano and Martin, 1988). After treatment, cellswere fixed, permeabilized, and stained with the appropriateantibody. Images were acquired using a microscope (Axioskop;Zeiss, Inc., Thornwood, NY) equipped with epifluorescence anda CCD camera (Photometrics Sensys, Tucson, AZ) using IP Labsoftware (Signal Analytics Corp., Vienna, VA). All images shownare the raw data collected at 1x1 binning with a gain of 1.

Lipid Synthesis Assays.
Cells were seeded onto 6-cm plastic dishes 2 d before the experimentso that they were 90% confluent the day of the experiment. Cellswere incubated in DME supplemented with 50 µg/ml cycloheximide,and half of the dishes were also incubated with 5 mM βCA.1 h later, fresh medium containing cycloheximide and [³H]palmitate(100 µCi/ dish) was added, along with either 1% isopropanol(control and βCA) or 100 µM PDMP and 5 mM βCAif indicated. 1 h later, cells were trypsinized and washedoff the plate in 0.8 ml cold PBS. To normalize lipid levels,50 µl were removed for a protein assay by the method ofBradford (1976). Lipids were then extracted by the method ofBligh and Dyer (1959). Labeled samples were doped with 10 µgcold ceramide to allow for visualization. Samples were runon 10 x 10 cm high performance thin-layer chromatography plateswith a mobile phase of chloroform/glacial acetic acid (9:1;Abe et al., 1992). Plates were sprayed with water to visualizethe ceramide bands that were scraped and counted after the addition of scintillation fluid. Alternatively, plates were dipped in10% 4,5-diphenyloxazole in chloroform for visualization by fluorography(Henderson and Tocher, 1992).

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Inhibition of Sphingolipid Synthesis by PDMP but Not βCA or FB1 Causes a Mislocalization of IBV M Protein to the ER
To test whether ongoing sphingolipid synthesis was necessaryfor the correct localization of the IBV M protein, we usedthree inhibitors of sphingolipid synthesis: β-chloroalanine(βCA; Medlock and Merrill, 1988), fumonisin B1 (FB1; Wang et al., 1991),and PDMP (Vunnam and Radin, 1980; Inokuchi and Radin, 1987).The biosynthetic pathway for sphingolipids with the sites ofinhibition of these drugs is shown in Fig. 1. Both βCA(5 mM) and FB1 (100 µM) inhibited the incorporation ofradiolabeled precursors into sphingolipids in BHK-21 cells by>90% (data not shown). Consistent with previous results(Rosenwald et al., 1992), we found that PDMP (100 µM)inhibited GlcCer synthesis by $~$ 90% and SM synthesis by $~$ 50% inBHK-21 cells (data not shown).

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Figure 1 Sphingolipid synthesis pathway. The pathway for sphingolipid biosynthesis in mammalian cells and the steps inhibited by the drugs used in this study are indicated.

To express the IBV M protein, BHK-21 cells were infected witha recombinant vaccinia virus encoding IBV M (Machamer and Rose, 1987).4 h after infection the cells were treated with cycloheximidefor 1 h to chase newly synthesized M protein out of the ER.Sphingolipid synthesis inhibitors were then added and the cellsincubated for another 1 h before processing for immunofluorescence (Fig. 2). In control cells, IBV M exhibited a tight, juxtanuclearstaining pattern that colocalized with Golgi markers. The Golgilocalization pattern of IBV M was unchanged by treatment witheither βCA or FB1, suggesting that ongoing sphingolipidsynthesis is not required for proper localization of IBV M.In contrast, PDMP-treated cells showed a marked change in thestaining pattern of the IBV M protein after 1 h. The localizationof IBV M in the presence of PDMP changed from Golgi to ER basedon the absence of strong juxtanuclear staining and the presenceof nuclear rim staining and a tubulo-reticular staining patternthat colocalized with ER markers. Treatment of infected cells with lower concentrations of PDMP had no effect on IBV M localizationand very little effect on SM synthesis (data not shown). Wenext tested the kinetics of PDMP-induced mislocalization ofIBV M. Cells were infected as before and treated for 1 h withcycloheximide. Then cells were treated with PDMP for varyinglengths of time up to 1 h (Fig. 3). Redistribution was firstobserved at 15 min and became maximal at 60 min. This redistributionwas rapidly reversible, such that 30 min after washing outPDMP, IBV M had moved back to the Golgi region.

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Figure 2 PDMP but not βCA or FB1 mislocalize IBV M to the ER. BHK-21 cells infected with a recombinant vaccinia virus encoding IBV M were treated 4 h after infection with 50 µg/ml cycloheximide for 1 h. Either 5 mM βCA, 100 µM FB1, or 100 µM PDMP was then added to the indicated samples for 1 h, at which time the cells were fixed and prepared for indirect immunofluorescence with antibodies directed against IBV M and Texas red secondary antibodies. For each experimental group, the Nomarski image is shown on the left and the fluorescence image on the right. Bar, 10 µm.

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Figure 3 The redistribution of IBV M induced by PDMP was rapid and reversible. BHK-21 cells infected with a recombinant vaccinia virus encoding IBV M were treated 4 h after infection with 50 µg/ml cycloheximide for 1 h. PDMP (100 µM) was added, and dishes were fixed at the indicated times and prepared for indirect immunofluorescence. After 1 h in PDMP, the remaining dishes were washed three times with 1 ml DME with serum and incubated with cycloheximide-containing medium for the indicated time before being prepared for indirect immunofluorescence. For each experimental series, the Nomarski image is shown on the left and the fluorescence image on the right. Bar, 10 µm.

PDMP Treatment Does Not Mislocalize Golgi Markers, but Does Mislocalize ERGIC-53
We next asked if PDMP mislocalized other Golgi markers. Cellswere infected and treated as described above and then stainedwith antibodies to two integral membrane proteins of the Golgistack, giantin (Linstedt and Hauri, 1993) and mannosidase II(Man II; Moremen and Robbins, 1991; Velasco et al., 1993). Treatmentof cells with 100 µM PDMP for 1 h had no effect on thelocalization of either protein (Fig. 4), suggesting that themorphology of the Golgi was not greatly altered. We also examinedthe localization of β-COP, a peripheral membrane proteinof the stack and CGN involved in vesicular traffic (Oprins et al., 1993).As seen in Fig. 4, the distribution of β-COP appeared unaffectedin treated cells.

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Figure 4 PDMP did not affect localization of endogenous Golgi markers. BHK-21 cells were incubated for 1 h with cycloheximide and then incubated for 1 h in medium with 1% isopropanol (control) or 100 µM PDMP. Cells were then fixed and prepared for indirect immunofluorescence with antibodies to Man II, giantin, or β-COP and Texas red secondary antibodies. For each experimental series, the Nomarski image is shown on the left and the fluorescence image on the right. Bar, 10 µm.

We then looked at a protein which cycles through the cis-Golgi.As we did not have access to antibodies that crossreact withknown markers in BHK-21 cells, we examined ERGIC-53 in Verocells. IBV M localizes to the CGN in these cells and is alsoredistributed to the ER by PDMP (data not shown). ERGIC-53is an IC protein that cycles between the ER, IC, and Golgistack (Lippincott-Schwartz et al., 1990; Schindler et al., 1993).Vero cells were treated with cycloheximide for 1 h and thenwith or without 100 µM PDMP for an additional hour beforebeing fixed and prepared for immunofluorescence (Fig. 5). Similarto the effects on IBV M, PDMP treatment shifted the steady-state distribution of ERGIC-53 to the ER. In addition, neither βCAnor FB1 had any effect on the localization of ERGIC-53 (datanot shown).

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Figure 5 PDMP induced the redistribution of the endogenous IC protein, ERGIC-53, to the ER. Vero cells were incubated with cycloheximide for 1 h and then incubated for 1 h in the presence either 1% isopropanol (control) or 100 µM PDMP. Cells were then fixed and prepared for indirect immunofluorescence with antibodies to ERGIC-53. For each experimental group, the Nomarski image is shown on the left and the fluorescence image on the right. Bar, 10 µm.

PDMP but Not βCA or FB1 Slows the Anterograde Traffic of VSV G
The above immunofluorescence results suggested that PDMP mightgenerally alter the distribution of proteins that have a dynamiclocalization mechanism. Interestingly, it has been shown thatPDMP slows the rate of both anterograde vesicular traffic (Rosenwald et al., 1992)and endocytosis (Chen et al., 1995) in CHO cells. We testedwhether PDMP also slowed anterograde traffic in BHK-21 cells.We used a plasma membrane protein, the well-characterized G protein from VSV. A pulse–chase experiment was performedeither in the presence or absence of PDMP, βCA, or FB1.The rate of accumulation of endo H–resistant VSV G wasused as an assay for the rate of arrival at the medial-Golgi.Neither βCA nor FB1 had any effect on the rate of anterogradetraffic. However, PDMP increased the half-time for transportby $~$ 2.5-fold from 18 to 44 min (Fig. 6).

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Figure 6 Effect of sphingolipid synthesis inhibitors on transit of VSV G to the medial-Golgi. BHK-21 cells were infected with VSV. At 3.25 h after infection, cells were incubated in the presence or absence of 5 mM βCA or 100 µM FB1. At 4 h after infection, cells were pulse labeled and chased in the presence or absence of 100 µM PDMP for the indicated times. Cells were lysed with detergent and VSV G was immunoprecipitated. After treatment of immunoprecipitates with endo H, samples were electrophoresed and autoradiographed. Scanning densitometry was used to quantitate the amount of endo H–resistant VSV G at each time point. The data shown are from one representative experiment. PDMP, but not βCA or FB1, slowed arrival of VSV G at the medial-Golgi by 2.5-fold. Pretreatment with either βCA or FB1 partially corrected the PDMP effect.

The PDMP Effect on Anterograde Traffic Is Ameliorated by Pretreatment with Either βCA or FB1
Fig. 6 shows that neither βCA nor FB1 had any effect on the transit rate of VSV G, suggesting that the decreased ratewith PDMP was not due to a block in the ongoing synthesis ofsphingolipids. PDMP inhibits the conversion of ceramide intoglycosphingolipids and sphingomyelin. One possible explanationfor the effects observed with PDMP was an accumulation of theprecursor ceramide. βCA and FB1 act upstream of PDMP (Fig.1), and the intermediates in sphingolipid synthesis betweenthese steps and ceramide production are thought to be shortlived (Merrill and Wang, 1986; Medlock and Merril, 1988). Toask if ceramide accumulation might mediate the PDMP-induced slowing of anterograde traffic, cells were treated with βCA or FB1 before PDMP. We performed a pulse–chase labelingexperiment with cells pretreated with either βCA or FB1for 1 h before being chased in the presence or absence of βCAor FB1 and PDMP (Fig. 6). Pretreatment with the earlier inhibitorsreduced the PDMP-induced slowing of anterograde traffic byabout half, suggesting that accumulation of newly synthesizedceramide at least partially mediates this effect.

Pretreatment with βCA or FB1 Reduces the PDMP-induced Mislocalization of IBV M Protein
To test whether ceramide was likely to mediate the PDMP-inducedmislocalization of IBV M, indirect immunofluorescence was performedas above with cells pretreated with either βCA or FB1for 1 h before the addition of PDMP. To simplify the quantification,the localization of IBV M was classified into one of threestaining patterns. Class 1 was the most commonly seen patternin untreated cells, i.e., tight juxta-nuclear staining thatcolocalized with Golgi markers. Class 3 was the most commonlyseen pattern in PDMP-treated cells, i.e., diffuse stainingwith prominent nuclear envelope staining that colocalized withER markers. Class 2 was intermediate between the class 1 andclass 3. Whether this pattern represents an overlap of ER and Golgi staining patterns or an increase in IC staining is not clear. For these experiments, coded samples were quantifiedby counting at least 100 cells for each sample. The experimentwas performed five times, with one representative experimentshown (Fig. 7). Interestingly, when cells were quantified inthis way, we observed that both βCA and FB1 caused a slightshift from class 1 to class 2. The significance of this observationis not clear. PDMP dramatically shifted the distribution ofIBV M from mainly class 1 in the control cells to mainly class3. Pretreatment with either βCA or FB1 significantly reducedthis shift in the staining pattern of IBV M, suggesting thataccumulation of newly synthesized ceramide mediates the effectsof PDMP on localization of IBV M.

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Figure 7 Effect of pretreatment with βCA and FB1 on PDMP-induced redistribution of IBV M. Cells were prepared for immunofluorescence as described in Fig. 2 with the exception that indicated samples were treated with either 5 mM βCA or 100 µM FB1 beginning with the cycloheximide chase 4 h after infection. At 5 h after infection, cells were treated with 1% isopropanol (control) or 100 µM PDMP. 1 h later the cells were fixed and prepared for indirect immunofluorescence. Random fields from coded samples were scored for the number of IBV M–expressing cells that fell into the three classes of staining pattern shown. Treating cells with FB1 or βCA before PDMP shifted the IBV M staining pattern towards the control pattern.

PDMP Increases Cellular Ceramide Levels
The pretreatment experiments suggested that increased levelsof ceramide mediate the PDMP-induced effects on IBV M localization.Ceramide can act as a second messenger (for review see Hannun, 1994)and has been suggested to be the mediator of some of the effectsof PDMP in CHO cells (Rosenwald and Pagano, 1993). Furthermore,in several systems, cellular levels of ceramide increased upon treatment with PDMP or one of its more soluble analogues (forexample see Rani et al., 1995; Posse de Chaves et al., 1997).We measured the levels of ceramide after various treatmentsby pulse–labeling with [³H]palmitate. After labeling andtreatment, cellular lipids were extracted and run on chromatographyplates. The appropriate spots corresponding to ceramide werescraped and counted. Consistent with our hypothesis, Fig. 8A shows that PDMP treatment increased the levels of ceramide2.5-fold over control levels. Pretreatment with βCA reducedPDMP- induced ceramide accumulation to roughly half of control levels, but this level was still threefold higher than cells treated with βCA alone. Fig. 8 B is a representative fluorographshowing the ceramide region that was quantified in Fig. 8 A.Interestingly, we noticed the appearance of a lower migratingceramide band in PDMP-treated cells.

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Figure 8 Treatment with PDMP increased the level of newly synthesized ceramide by 2.5-fold. BHK-21 cells were incubated with 50 µg/ml cycloheximide and, if indicated, 5 mM βCA. After 1 h, media was replaced with medium containing cycloheximide, 100 µCi [³H]palmitate (50 Ci/mmol), βCA if indicated, and either 1% isopropanol (control and βCA) or 100 µM PDMP. After 1 h, cells were trypsinized to remove them from the dish and the lipids were extracted as described. (A) The spots corresponding to ceramides on the chromatography plates were scraped, extracted, and counted. Four experiments were performed, with duplicate plates for each. Shown are the mean values ± SEM. (B) A representative fluorogram showing the ceramide region of the chromatography plate.

A Soluble Analogue of Ceramide Does Not Affect the Localization of IBV M or ERGIC-53
The pretreatment experiments as well as lipid analysis implicatedceramide as the mediator of PDMP effects. If this were true,addition of a soluble, short-chain analogue of ceramide mightmimic the effects of PDMP. Indeed, one such cell-permeableanalogue of ceramide, N-hexanoylsphingosine (C₆Cer), reproducesthe effects of PDMP on anterograde traffic of VSV G in CHO cells(Rosenwald and Pagano, 1993). We first asked whether C₆Cerslowed anterograde traffic in BHK-21 cells. A pulse–chaselabeling experiment with VSV-infected cells was performed,with cells chased in the absence or presence of 25 µMC₆Cer. C₆Cer slowed the rate of anterograde traffic in BHK-21 cells $~$ 2.5-fold (data not shown). We went on to use C₆Cer inour indirect immunofluorescence assay. As expected, C₆Cer hadno effect on the localization of either Man II or β-COP(Fig. 9). However, contrary to our expectation, C₆Cer did notalter the localization of either IBV M or ERGIC-53. This suggeststhat exogenously added C₆Cer and ceramide generated by treatmentwith PDMP do not have the same effects. Two other soluble analoguesof ceramide, C₂Cer and C₈Cer, were also tested and found tohave no effect on the localization of IBV M (data not shown).

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Figure 9 Exogenous C₆Cer did not redistribute IBV M or ERGIC-53. BHK cells (IBV M, Man II, and β-COP) or Vero cells (ERGIC-53) were infected with a recombinant vaccinia virus expressing IBV M. 4 h after infection the cells were treated with 50 µg/ml cycloheximide. At 5 h after infection cells were incubated for 1 h in serum-free DME with 0.34 mg/ml defatted BSA with or without 25 µM C₆Cer. Cells were then prepared for indirect immunofluorescence and stained with the indicated antibodies. For each experimental series, the Nomarski image is shown on the left and the fluorescence image on the right. Bar, 10 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Steady-State Localization of IBV M Involves Cycling through the ER
There are two possible mechanisms to maintain the steady-statelocalization of proteins to specific sites along the secretorypathway: (a) retention in the particular compartment, and (b)retrieval from other compartments (Machamer, 1993; Nilsson and Warren, 1994).The redistribution of IBV M induced by PDMP was surprising,as we expected that if we disrupted its localization, it would move with "bulk flow" to the plasma membrane. That IBV M wasredistributed to the ER suggests that it has specific targetinginformation for retrieval to the ER. Coupled with earlier workin our laboratory on the role of oligomerization of IBV M chimerasin CGN targeting (Weisz et al., 1993), our findings suggestthat IBV M maintains its steady-state distribution by bothretention and retrieval (Fig. 10 A). We propose two modelsto explain the redistribution of IBV M protein induced by PDMP.The simplest model (Fig. 10 B, left arrow) is that the M protein normally cycles between the ER and the Golgi at a significantrate, as has been shown for ERGIC-53 (Lippincott-Schwartz et al., 1990;Schindler et al., 1993). The slowing of anterograde trafficwould cause the protein to shift its steady-state distributionto the ER, assuming that retrograde traffic is unaffected orperhaps increased by PDMP. A second possibility is that PDMPdisrupts retention of the M protein, which then cycles backto the ER by normal retrieval mechanisms (Fig. 10 B, rightarrow). These two models are not mutually exclusive, and botheffects of PDMP may be necessary to redistribute IBV M to theextent observed.

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Figure 10 Current models for how IBV M maintains its steady-state distribution and how PDMP might alter this distribution. (A) Evidence presented here shows that IBV M can be induced to redistribute to the ER, indicating that IBV M has information necessary for traffic to the ER. We propose that IBV M normally maintains its steady-state distribution by cycling through the ER at some basal rate. (B) If IBV M is cycling through the ER normally, then its localization would depend on the balance of anterograde and retrograde traffic rates. As PDMP slows anterograde traffic, IBV M could accumulate in the ER when the balance of membrane traffic is disrupted (left arrow). Alternatively, PDMP may act by disrupting the retention of IBV M, causing it to move out of the Golgi (right arrow). It is also possible that redistribution of IBV M requires both effects of PDMP.

Implicit in both models is the idea that IBV M contains retrievalinformation. PDMP-induced ER redistribution was also observedfor ERGIC-53, a dilysine-containing IC marker known to cyclethrough the ER (Lippincott-Schwartz et al., 1990; Schindler et al., 1993).Double-label immunoelectron microscopy in HeLa cells showedthat the distribution of ERGIC-53 and IBV M overlapped significantly, though not completely (Sodeik et al., 1993). This suggests that IBV M may in part use the same, as yet unknown, cellularmachinery used by IC proteins to maintain its steady- statelocalization. Using deletion mutants and chimeric molecules,dissection of IBV M retention and retrieval information shouldbe possible using PDMP as a tool. The pathway followed by IBVM during retrieval will also be important to decipher. Experimentsin nontreated cells suggest that the protein may move throughlater Golgi compartments even though its steady-state distributionis the CGN, because its oligosaccharides are slowly processed(Machamer et al., 1990).

Interestingly, we did not observe redistribution of two Golgistack markers (Man II and giantin) to the ER with PDMP treatment.Golgi membrane proteins were recently suggested to be highlymobile (Cole et al., 1996b) and to cycle through the ER (Cole et al., 1996a).Our results with PDMP suggest that cycling of these proteinsdoes not occur during the time scale of our experiments, and/orthat its predominant effect on IBV M is a loss of retention.

Ceramide Mediates the Effects of PDMP
Interestingly, it has been shown that myriocin, an inhibitor of sphingolipid synthesis thought to inhibit the same step as βCA, reduces the rate of transport of a glycosylphosphatidylinositol-linkedprotein but not other proteins out of the ER in yeast (Horvath et al., 1994).It would be interesting to test whether inhibition of ceramidesynthesis in mammalian cells also slows the rate of transportof glycosylphosphatidylinositol-linked proteins in mammaliancells. However, neither βCA nor FB1 had an effect on therate of anterograde traffic of VSV G or the localization ofIC, CGN, or Golgi stack proteins. When we quantified the effectsof these two inhibitors on the immunofluorescence stainingpattern of IBV M, we did detect a slight shift toward the intermediatestaining pattern (Fig. 7). Whether this represents an altereddistribution pattern or subtle effects on Golgi structure causedby these inhibitors is unclear. From these results we concludethat ongoing sphingolipid synthesis is not required for eithernormal rates of anterograde traffic or proper localizationof Golgi proteins. However, the glucosylceramide analogue PDMP,at a concentration that inhibits both GlcCer and SM synthases, causes a redistribution of IBV M to the ER and a slowing ofanterograde traffic in BHK-21 cells. Why does PDMP have theseeffects while βCA and FB1 do not? It is likely that PDMPexerts its effects by causing the accumulation of ceramide.Other groups have found that the various effects of PDMP andits active analogues were concomitant with (Uemura et al., 1990;Shayman et al.; 1991; Rani et al., 1995) or actually causedby increases in ceramide concentrations (Abe et al., 1996; Posse de Chaves et al., 1997).In BHK-21 cells treated with 100 µM PDMP for 1 h we measuredan increase in newly synthesized ceramide (Fig. 8 A), showingat least a correlation between levels of newly synthesized ceramideand the effects of PDMP on protein traffic and localization.The fact that pretreatment with either βCA or FB1, bothof which block the synthesis of ceramide, can ameliorate theeffects of PDMP demonstrates that ceramide is at least in partthe mediator of these effects. However, the effects of PDMPare not completely abolished by pretreatment, even though βCApretreatment reduced the level of newly synthesized ceramideby 50% compared to control. One explanation is that ceramideaccumulation is only one of the ways that PDMP exerts its effects.Another possibility is that ceramide is being generated by thedegradation of preexisting sphingolipids, e.g., at the cellsurface or in lysosomes. This ceramide cannot be made back intosphingolipids because the enzymes SM and GlcCer synthases areinhibited in the presence of PDMP. Interestingly, the fluorographof the ceramide bands generated after the various treatments(Fig. 8 B) shows different relative amounts of ceramide species. We suspect that these ceramides differ in acyl chain lengths (Abe et al., 1992) and that this may be an indication of differentsources of ceramide, i.e., de novo synthesis or sphingolipiddegradation. We are currently investigating this possibility.

Accumulation of Endogenous Ceramide by PDMP Treatment and Exogenous C₆Cer Do Not Have the Same Effects
Based on the pretreatment results, we expected that solubleanalogues of ceramide would mimic the effects of PDMP. Rosenwald and Pagano (1993)showed that like 100 µM PDMP, 25 µM C₆Cer decreasedthe rate of transit of an itinerant protein to the medial-Golgiin CHO cells. Consistent with these results, 25 µM C₆Ceralso slowed anterograde traffic in BHK-21 cells. However, 25µM C₆Cer had no effect on the localization of eitherthe M protein or ERGIC-53. Other short-chain ceramide analogues(C₂- and C₈-ceramide) also had no effect on IBV M localization.How does this fit with our model that ceramide mediates PDMPeffects? One explanation is that the effect on protein localizationis independent of the effect on anterograde traffic rates. Inthis case, it may be that C₆Cer and endogenous ceramide havesimilar ability to bind and affect proteins that regulate anterogradetraffic, but C₆Cer is unable to bind or affect proteins thatregulate protein localization. It has been shown that some shortchain analogues of ceramide do not have the same effects asendogenous ceramide (e.g., Wolff et al., 1994). A second possibility is that effects of ceramide are limited to the bilayers in which its concentration increases, and the difference seen between endogenous ceramide and exogenous C₆Cer is due tothe different intracellular distribution of these molecules.C₆Cer would be unlikely to accumulate in compartments whereIBV M and ERGIC 53 reside, because it is rapidly convertedto sphingolipids there (Rosenwald et al., 1992). Effects onmembrane traffic might be more dramatic in compartments whereC₆Cer accumulates, possibly the trans-Golgi and TGN (Pagano et al., 1989).Consistent with this idea, the rate of movement of VSV G throughthe late Golgi (measured by sialylation) was slowed to a much greater extent by C₆Cer than by PDMP (Rosenwald and Pagano, 1993).

It is not yet clear how ceramide induces the changes in anterogradetraffic and protein localization. Recent studies have shownthat ceramide (Hannun, 1994) and its metabolites (Hakomori, 1990)play a major role as second messengers. Preliminary experimentswith both the ceramidase inhibitor N-oleoylethanolamine andexogenously added sphingosine suggest that the ceramide breakdown product sphingosine does not play a role in the localization of IBV M (Maceyka, M., and C. Machamer, unpublished observations).Ceramide activates a cytosolic protein phosphatase (Dobrowsky and Hannun, 1992;Wolff et al., 1994) that can be inhibited by okadaic acid.Preliminary experiments suggest that okadaic acid does not blockthe PDMP-induced changes (Maceyka, M., and C. Machamer, unpublishedobservations). Ceramide could be activating a protein kinase(Mathias et al., 1991), but this kinase has not been fullycharacterized. Another possibility is that increased ceramidewithin the lipid bilayer directly affects the localization ofIBV M. Earlier work from our laboratory showed that the firsttransmembrane domain of IBV M can target chimeras to the CGN(Swift and Machamer, 1991; Machamer et al., 1993). It is possiblethat CGN bilayers have distinct lipid domains, and that thesedomains contain different sets of proteins, analogous to glycosphingolipidrafts. Segregation of membrane proteins involved in vesiculartraffic, such as SNAREs, would lead to mobile and immobiledomains. We hypothesize that under normal conditions, IBV Mwould be targeted to an immobile domain and escaped moleculeswould be cycled back through the ER. Elevated levels of ceramidecould disrupt these immobile lipid domains, inducing IBV M tocycle. Alternatively, perhaps ceramide binds to IBV M transmembranedomains, preventing an interaction with immobile lipid domains.

Acknowledgments

We thank Drs. E. Cluett, D. Raben, and A. Hubbard for usefuldiscussions and the members of the Machamer lab for criticalreading of the manuscript. We also thank H.-P. Hauri, M. Farquhar,K. Moremen, and J. Lippincott-Schwartz for antibodies.

This work was supported by grant GM42522 from the National Institutesof Health.

Submitted: 29 August 1997

Revised: 6 October 1997

Address all correspondence to Carolyn E. Machamer, Departmentof Cell Biology and Anatomy, Johns Hopkins University Schoolof Medicine, 725 N. Wolfe St., Baltimore, MD 21205. Tel.: (410)955-1809. Fax: (410) 955-4129. E-mail: carolyn_machamer{at}qmail.bs.jhu.edu

References

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Abstract
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References

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