Rhabdoviruses and the Cellular Ubiquitin-Proteasome System: a Budding Interaction

doi:10.1128/JVI.75.22.10623-10629.2001

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Journal of Virology, November 2001, p. 10623-10629, Vol. 75, No. 22
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.22.10623-10629.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Rhabdoviruses and the Cellular Ubiquitin-Proteasome System: a Budding Interaction

Ronald N. Harty,¹^,^* Melissa E. Brown,¹ James P. McGettigan,² Guangli Wang,³^, Himangi R. Jayakar,⁴ Jon M. Huibregtse,³ Michael A. Whitt,⁴ and Matthias J. Schnell²

Department of Pathobiology, School of Veterinary Medicine, University of Pennsylvania, Philadelphia, Pennsylvania 19104¹; Department of Biochemistry and Molecular Pharmacology, Center for Human Virology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107²; Department of Molecular Genetics and Microbiology, University of Texas at Austin, Austin, Texas 78712³; and Department of Molecular Sciences, University of Tennessee-Memphis, Memphis, Tennessee 38163⁴

Received 28 June 2001/Accepted 8 August 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The matrix (M) proteins of vesicular stomatitis virus (VSV) and rabies virus (RV) play a key role in both assembly and buddingof progeny virions. A PPPY motif (PY motif or late-budding domain)is conserved in the M proteins of VSV and RV. These PY motifsare important for virus budding and for mediating interactionswith specific cellular proteins containing WW domains. The PYmotif and flanking sequences of the M protein of VSV were usedas bait to screen a mouse embryo cDNA library for cellular interactors.The mouse Nedd4 protein, a membrane-localized ubiquitin ligasecontaining multiple WW domains, was identified from this screen.Ubiquitin ligase Rsp5, the yeast homolog of Nedd4, was able tointeract both physically and functionally with full-length VSVM protein in a PY-dependent manner. Indeed, the VSV M proteinwas multiubiquitinated by Rsp5 in an in vitro ubiquitination assay.To demonstrate further that ubiquitin may be involved in the buddingprocess of rhabdoviruses, proteasome inhibitors (e.g., MG132)were used to decrease the level of free ubiquitin in VSV- andRV-infected cells. Viral titers measured from MG132-treated cellswere reproducibly 10- to 20-fold lower than those measured fromuntreated control cells, suggesting that free ubiquitin is importantfor efficient virus budding. Last, release of a VSV PY mutantwas not inhibited in the presence of MG132, signifying that thefunctional L domain of VSV is required for the inhibitory effectexhibited by MG132. These data suggest that the cellular ubiquitin-proteasomemachinery is involved in the budding process of VSV andRV.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The Rhabdoviridae represent a divergent and complex family of negative-sense RNA viruses, of which Vesicular stomatitis virus(VSV) and Rabies virus (RV) are members. VSV maintains a minimalgenome encoding five structural proteins: N (nucleoprotein), P(phosphoprotein), M (matrix protein), G (glycoprotein), and L(polymeraseprotein).

The M protein is an abundant, multifunctional virion protein that plays a role in gene regulation, cellular pathogenesis,and, along with the G protein, virion assembly and budding (2,6, 7, 10, 14, 20, 23, 29, 30, 41, 43). Animportant characteristic of the M protein of VSV, shared by theGag polyprotein of retroviruses (1, 12, 36, 39, 57,59, 60) and the VP40 protein of Ebola virus (13, 19, 52),is its ability to be released (bud) from cells in the absenceof any other viral protein (14, 21, 27). Recent investigationsinto this budding function exhibited by the M protein revealedthat a proline-rich region (PPPY or PY motif) conserved at theN terminus of M was critical for efficient budding (7, 14).Indeed, infectious VSV PY mutants were significantly impairedin their ability to separate completely (pinch off) from the plasmamembranes of infected cells (20). The PY motif has been termeda late-budding domain (L domain) for its involvement in a latestep of the budding process. The conservation of functional Ldomains in members of the Rhabdoviridae, Retroviridae, and Filoviridaefamilies is now well documented (1, 7, 13, 14, 20,33, 36, 39, 45, 49, 57, 59, 60). While the premisethat these divergent RNA viruses may utilize common machineryto break out of cells remains intriguing, the mechanism by whichthese L domains accomplish this task remainsunknown.

It has been postulated previously that viral L domains may mediate their function via an interaction with a cellular protein(s).This insight was initiated by Garnier et al. (12), who demonstratedthat the PY motif of the Rous sarcoma virus (RSV) Gag mediatedinteractions in vitro with one of the WW domains present withincellular protein YAP. Unlike SH3 domains, which prefer core consensussequence PxxP, type I WW domains prefer core consensus sequencePPxY (24, 50, 51). To date, four different types of WW domainshave been identified in a wide range of cellular proteins havingvarious functions, and the PY motifs of RSV Gag, VSV M, RV M,and Ebola virus VP40 proteins have been shown to interact withspecific, type I WW domain-containing proteins (12-14, 51).

One family of cellular proteins that contain multiple WW domains and that interact strongly with viral PY motifs are E3 ubiquitinligases (e.g., Nedd4/Rsp5) (13, 14, 28, 58). The mammalianNedd4 protein and its homolog in yeast, Rsp5, are membrane-localizedubiquitin ligases that play a role in endocytosis (3, 8,9, 11, 15-18, 22, 25, 26, 38, 42, 47, 54, 55).While ubiquitination often targets a protein for degradation bythe 26S proteasome, increasing evidence suggests that ubiquitination,in particular, monoubiquitination, may be a signal for somethingother than degradation (e.g., endocytosis) (4, 5, 8,9, 16, 42, 46, 54).

Recent findings have implicated free ubiquitin and ubiquitin ligases as being integral components of the budding machineryof retroviruses and perhaps of filoviruses (13, 37, 45,49, 53). In this report, we present evidence that the cellularubiquitin-proteasome machinery is influential in the budding processof VSV and RV. Our results indicate that the VSV M protein caninteract both physically and functionally with the Rsp5 ubiquitinligase in a PY-dependent manner. Moreover, the release of bothinfectious VSV and RV from infected cells was decreased significantlyin the presence of proteasome inhibitors, which reduce the levelof free ubiquitin in treated cells (31). In contrast, releaseof a VSV PY mutant was not affected by proteasomeinhibitors.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses and cells. VSV (Indiana serotype) was propagated and titered on BHK-21 cells, which were maintained in Dulbecco modified essential medium(DMEM) (Life Technologies, Rockville, Md) supplemented with 10%fetal calf serum (HyClone) and penicillin-streptomycin (Life Technologies).BSR-T7 cells were kindly provided by K.-K. Conzelmann (Max-von-PettenkoferInstitut, Munich, Germany). BSR-T7 cells were maintained as describedabove with the addition of 1.0 mg of G-418 (Mediatech, Herndon,Va.)/ml every second or thirdpassage.

Plasmids and antibodies. The wild-type M gene of VSV (Indiana serotype) was subcloned from vector pSP72 (14) by PCR using primers flanking the entireopen reading frame. The PCR product was then inserted into thepYES2 vector (Invitrogen, Carlsbad, Calif.) using SacI/XhoI restrictionendonuclease sites to generate pYESMWT. A PY mutant form of VSVM (PPPY changed to AAAA) (14) was also cloned into the SacI/XhoIsites of the pYES2 vector to generate pYESMA4. Plasmids APVSVMWTand APVSVMA4 encoding VSV M and bacterial alkaline phosphatasefusion proteins have been described previously (2). PlasmidGST-Rsp5 encodes a fusion protein consisting of full-length Rsp5joined to the glutathione S-transferase moiety. Monoclonal antibody23H12 specific for the M protein of VSV was kindly provided byD. S. Lyles (Bowman-Gray School of Medicine, Winston-Salem, N.C.).

cDNA library screen. A $lambda$ Exlox cDNA library (Novagen) from a 14-day-old mouse embryo was screened for proteins that interacted with amino acids(aa) 17 to 33 of the VSV M protein in accordance with the protocolof thesupplier.

Proteasome inhibitors and VSV budding. MG132, MG115, lactacystin, and epoxomycin were obtained from Calbiochem and suspended in dimethyl sulfoxide (DMSO) as indicatedby the supplier. The suspended inhibitors were stored at $-$ 20°Cand used within a 2-week period. BSR-T7 cells were infected withVSV at a multiplicity of infection (MOI) of 3.0 for 1 h at 37°C.The inoculum was removed, and the cells were washed with 1× phosphate-bufferedsaline. Normal medium was added to the cells, and the infectionwas allowed to proceed for 3 h at 37°C. DMSO alone or proteasomeinhibitors at concentrations indicated in Results were added tothe appropriate dishes, and the infection was allowed to proceedup to an additional 2.5 h. Supernatants were harvested and storedat $-$ 80°C. Serial dilutions of virus-containing supernatants wereused to infect fresh monolayers of either BSR-T7 or BHK-21 cellsin 35-mm-diameter dishes. Mock-infected and infected cells wereoverlaid with 1.0% methylcellulose and allowed to incubate upto 48 h at 37°C. VSV titers reported represent averages of sixindependent experiments. For the time course analysis, the initialMOI was 1.0 PFU/ml and 50 µM MG132 was added to the media at 5.5hpostinfection.

Proteasome inhibitors and RV budding. BSR-T7 cells were plated in six-well plates and infected at an MOI of 10 with recombinant RV SBN (44). Sixteen hours postinfection,cells were washed with DMEM supplemented with 10% serum. Two millilitersof DMEM plus 10% serum containing 100 µM MG132 diluted in DMSOor DMSO alone was added to the monolayers for 2.5 h. Supernatantswere collected, and infectious titers were determined in duplicateon BSR cells. For protein synthesis control studies, BSR cellswere plated in 25 cm² flasks and infected with recombinant RV SBN at an MOI of 10 for16 h. Monolayers were washed in methionine-free media and thenmetabolically labeled for 2.5 h with 250 µCi of [³⁵S]methionine in the presence of 100 µM MG132 or DMSO alone. Supernatantswere collected, and virions were purified through 10% sucrosefor 1 h at 20,000 rpm. The viral pellet was suspended in 50 µlof protein lysis buffer. Cells were washed in 1× phosphate-bufferedsaline and then lysed in lysis buffer (50 mM Tris [pH 7.4], 150mM NaCl, 1.0% Nonidet P-40, 0.1% sodium dodecyl sulfate [SDS],1× protease inhibitor [Sigma]) on ice for 5 min. Proteins fromsupernatants and cell lysates were analyzed by SDS-10% polyacrylamidegel electrophoresis (PAGE) and visualized by a phosphorimager(MolecularDynamics).

Immunoprecipitation analysis. For immunoprecipitation analysis, 100 µCi of ³⁵S-Express label (NEN DuPont) was added to each monolayer concomitant with theaddition of the proteasome inhibitor. Cell extract and supernatantsamples were immunoprecipitated with monoclonal antibody 23H12against the VSV M protein and analyzed as described previously(13, 14). Immunoprecipitated proteins were visualized by autoradiographyand quantitated using a phosphorimager (Bio-Rad; GS-525 molecularimager system). These experiments were repeated at least threetimes.

Far-Western blotting. Plasmids GST-Rsp5, APVSVMWT, and APVSVMA4 were used in this assay. Far-Western blotting was performed as described previously(14).

Ubiquitination assay. Plasmids pYESMWT and pYESMA4 were employed in this assay. The positive control for this assay was the 52-kDa yeast proteinencoded by the YHL002w gene (G. Wang and J. Huibregtse, unpublisheddata). In vitro ubiquitination assays were performed as describedpreviously (13, 18).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

cDNA library screen with the PY motif of VSV M protein. The PY motifs conserved in the M protein of VSV and RV, the VP40 protein of Ebola virus, and the Gag protein of RSV were shownto mediate interactions with WW domains of several cellular proteins(12-14). To extend these observations, a mouse cDNA library ( $lambda$ Exlox)was screened using the PY motif and flanking sequences (aa 17to 33) from VSV M as the probe. One of the cellular proteins isolatedfrom this screen was identified by DNA sequencing analysis asthe mouse Nedd4 gene, which contains three WW domains (GenBankaccession no. D85414; Fig. 1). The cDNA insert contained aa46 to 958 (Fig. 1). The WW domains from the mNedd4 protein wereshown previously to interact strongly with the PY motifs of theM proteins of VSV and RV (14). These results lend further supportto our hypothesis that the cellular Nedd4 ubiquitin ligase maybe an important component of the budding machinery of VSV andRV.

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FIG. 1. Schematic diagram of mNedd4 cDNA. Shaded boxes, presence and approximate locations of the three WW domains. Amino acids 46 to 958 are present within the cDNA insert.

Functional interaction between full-length VSV M and full-length Rsp5 ubiquitin ligase. The Nedd4 ubiquitin ligase represents a realistic candidate for a cellular interactor that may facilitate the budding processof VSV for the following reasons. (i) Nedd4 was isolated froma cDNA library screen (above), and its WW domains interact stronglywith viral PY motifs (14). (ii) Nedd4 is localized to the plasmamembrane of the cell, where it functions in endocytosis and ubiquitination(3, 38, 42). (iii) Recent studies have implicated ubiquitinand ubiquitin ligases as being important in retrovirus and perhapsfilovirus budding (13, 37, 45, 49, 53).

The functional homolog of Nedd4 in yeast is Rsp5, a membrane-associated ubiquitin ligase that contains multiple WW domainsand that functions in endocytosis. We made use of an establishedin vitro ubiquitination assay to address whether full-length VSVM could be ubiquitinated by full-length Rsp5 (Fig. 2A). The pYESMWTand pYESMA4 plasmids were used to synthesize wild-type VSV M proteinand a mutant M protein containing four alanines in place of PPPYin vitro, respectively. The radiolabeled wild-type M protein wasadded for the in vitro ubiquitination assays (performed in duplicate)in the presence (Fig. 2A, lanes 5 and 6) or absence of enzymaticallyactive Rsp5 (Fig. 2A, lanes 3 and 4). In the presence of Rsp5,numerous higher-molecular-weight species of multiubiquitinatedM protein were markedly evident, along with a concomitant decreasein unmodified VSV M (Fig. 2A, lanes 5 and 6). Ubiquitinated formsof wild-type VSV M were not observed in the absence of Rsp5 (lanes3 and 4). In stark contrast to what was found for wild-type M,no ubiquitination of the VSV M A4 mutant was detected in the absence(Fig. 2A, lanes 7 and 8) or presence (lanes 9 and 10) of Rsp5.These results demonstrate that full-length VSV M (wild type) caninteract both physically and functionally with full-length Rsp5in vitro.

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FIG. 2. Physical and functional interactions between VSV M and Rsp5. (A) Full-length VSV M was transcribed and translated in vitro in the presence of [³⁵S]methionoine and incubated with ATP, ubiquitin, E1 enzyme, and E2 protein (UBC8 from Arabidopsis thaliana).+, reactions with wild-type (WT) Rsp5 (lanes 2, 5, 6, 9, and 10); $-$ , reactions without WT Rsp5 (lanes 1, 3, 4, 7, and 8). The positions of unmodified WT VSV M (lanes 3 to 6) and of the unmodified VSV A4 mutant (lanes 7 to 10) are indicated. Multiubiquitinated forms of WT VSV M [M-ub(n)] are shown (lanes 5 and 6). A yeast protein of approximately 52 kDa encoded by the YHL002w gene is shown as a positive control for ubiquitination by Rsp5 (lanes 1 and 2). (B) Far-Western binding assay. Two micrograms of GST-Rsp5 (full-length Rsp5) were immobilized onto nitrocellulose filters and probed with BAP-VSV M (WT) or BAP-VSV M (A4 mutant).

To further support the specificity of the physical interaction between VSV M and Rsp5, a far-Western assay was performed (Fig.2B). Full-length Rsp5 joined to glutathione S-transferase waspurified from Escherichia coli and immobilized onto nitrocellulosefilters. Identical filters were probed with either full-lengthwild-type VSV M or the A4 mutant form of VSV M (Fig. 2B). As indicated,the wild-type M protein interacted with Rsp5, whereas the A4 mutantdid not (Fig. 2B).

Proteasome inhibitors block release of VSV. Since the VSV M protein was readily modified by ubiquitin in vitro, we wanted to determine whether alterations of free-ubiquitinlevels in the cell would affect the release of progeny VSV. Inhibitorsthat block the function of the proteasome (e.g., MG132) resultin a decrease in the level of free ubiquitin in the cytoplasm(31, 37, 45). BSR-T7 cells were infected with VSV, and,at 4 h postinfection, either DMSO alone or 50 µM MG132 solubilizedin DMSO was added to the cells for 2.5 h. Supernatants containingnewly released virions were collected and assayed for infectiousvirus by plaque titration (Fig. 3A). The titers of VSV illustratedrepresent the averages of six independent experiments (Fig. 3A).In the absence of MG132, newly released VSV achieved an averagetiter of 2.2 × 10⁸ PFU/ml, while, in the presence of 50 µM MG132, newly releasedVSV achieved an average titer of 2.0 × 10⁷ PFU/ml (Fig. 3A). This decrease in titer of slightly more than1 log unit was highly reproducible, and a similar decrease intiter was observed in the presence of other proteasome inhibitors(e.g., MG115, lactacystin, and epoxomycin; data not shown).

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FIG. 3. Inhibition of VSV release by MG132. (A) Titers of VSV present in the supernatant of cells infected in the absence ( $-$ ) or presence (+) of MG132 (50 µM). VSV titers and standard deviations represent averages of six independent experiments. (B) Time course analysis of VSV replication. Viral titers were determined from supernatant samples harvested at the indicated time points from cells infected in the presence or absence of MG132 (50 µM). MG132 was added to VSV-infected cells at 5.5 h postinfection (arrowhead). (C) Immunoprecipitation of radiolabeled VSV M protein from cell extracts (cells, lanes 1 and 2) and supernatants (media, lanes 1 and 2) of cells infected in the absence ( $-$ ) or presence (+) of MG132 (50 µM).

VSV release from cells incubated in the presence or absence of MG132 was measured during a time course experiment (Fig. 3B).MG132 (50 µM) or DMSO was added to the media 5.5 h postinfection(Fig. 3B). Release of VSV was inhibited in a time-dependent mannerimmediately following the addition of MG132 (Fig. 3B), comparedto that of VSV in the presence of DMSO alone (Fig. 3B). The differencein VSV titers at 9 h postinfection was approximately 10-fold (5.0× 10⁷ versus 5.6 × 10⁶ PFU/ml), consistent with results shown in Fig. 3A.

VSV-infected cells were incubated with proteasome inhibitors for no more than 2.5 h since prolonged exposure to these inhibitorscan lead to a complete shutdown of protein synthesis. To demonstratethat total protein synthesis in the above experiments was notadversely affected by MG132, radiolabeled viral proteins frominfected-cell extracts and supernatants were subjected to immunoprecipitation(Fig. 3C). Equivalent amounts of cell extracts infected with VSVin the absence (Fig. 3C, lane 1 cells) or presence (lane 2 cells)of MG132 were immunoprecipitated with monoclonal antibody 23H12against the VSV M protein. Virtually identical amounts (<2.0-folddifference) of M protein were present in cells treated with eitherDMSO or MG132 (Fig. 3C). In contrast, the amount of M proteindetected in the supernatant (Fig. 3C, lane 2 media) of MG132-treatedcells was reduced by approximately 12-fold compared to that detectedin the supernatant of DMSO-treated cells (Fig. 3C, lane 1 media).These data demonstrate that, under these experimental conditions,MG132 did not affect protein synthesis but rather specificallyinhibited the release of progeny virions as determined by bothvirus titration andimmunoprecipitation.

Proteasome inhibitors block release of RV. Since the PY motif is conserved in the M protein of RV and since the RV PY motif also mediates interactions with cellularproteins, we reasoned that release of RV would also be affectedby proteasome inhibitors. RV was used to infect monolayers ofBSR cells, and MG132 or DMSO was added at 16 h postinfection sincethe kinetics of RV replication and release are slower that thoseof VSV. As with VSV, RV-infected cells were incubated with MG132for no more than 2.5 h. The average RV titers from three independentexperiments performed in duplicate were 1.2 × 10⁷ PFU/ml in the presence of DMSO alone (Fig. 4B) and 7.0 × 10⁵ PFU/ml in the presence of 100 µM MG132 (Fig. 4B). This 16-foldreduction in virus titer is similar to those observed for VSVin the presence of 50 µM MG132 (10-fold; shown above) and 100µM MG132 (>20-fold; data not shown). To ensure that the observeddecrease in RV titer was not due to general inhibition of proteinsynthesis by MG132, radiolabeled proteins from both RV-infectedcell extracts and supernatants were examined by SDS-PAGE (Fig.4A). In two independent experiments, total protein synthesis incell lysates treated with DMSO alone was shown to be identicalto that in cells treated with 100 µM MG132 (Fig. 4A). In contrast,radiolabeled RV proteins (G, N, and M) present in the supernatantsfrom cells treated with DMSO alone were readily detected followingSDS-PAGE, whereas those present in supernatants from cells treatedwith MG132 were not detected in this assay (Fig. 4A). These resultsare highly consistent with those described above for VSV. Theseresults indicate that inhibitors of the cellular proteasome machineryimpair the budding efficiency of VSV and RV.

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FIG. 4. Inhibition of RV release by MG132. (A) Protein gel depicting radiolabeled proteins from both supernatants and cell lysates. Protein patterns from cells infected in the absence ( $-$ ) or presence (+) of MG132 (100 µM) are shown in duplicate. The G, N, and M proteins of RV are readily visible in supernatant samples from cells infected in the absence of MG132 but are not readily visible in supernatant samples from cells infected in the presence of MG132. (B) Titers of RV present in the supernatants of cells infected in the absence ( $-$ ) or presence (+) of MG132 (100 µM). RV titers and standard deviations represent averages of three independent experiments.

Release of a VSV PY mutant is not blocked by MG132. It has been postulated that inhibition of human immunodeficiency virus type 1 (HIV-1) budding by proteasome inhibitors isdependent on the presence of both the functional L domain (PTAPP)within the p6 region of Gag and the protease (PR) function ofHIV-1 Gag (45). To determine whether inhibition of VSV buddingby proteasome inhibitors is linked to the presence of the PY motifwithin the VSV M protein, we employed a VSV PY mutant. Recoveryof a budding-defective VSV PY mutant containing the sequence AAPA(AAPA virus) in place of PPPY was reported recently (20). Wehypothesized that the AAPA virus may be insensitive to the presenceof proteasome inhibitors for the following reason. Since the AAPAmutant would likely be impaired in its ability to interact withcellular WW domains of ubiquitin ligases (e.g., Nedd4), it wouldnot be ubiquitinated efficiently. Therefore, the reduction offree ubiquitin in infected cells due to MG132 should have no effecton release of the AAPA virus. To test this hypothesis, the AAPAvirus was used to infect monolayers of BHK-21 cells in the presenceof DMSO alone or 50 µM MG132 as described above for wild-typeVSV. The average titer of AAPA virus from the supernatants ofcells infected in the presence of DMSO alone was 3.2 × 10⁶ PFU/ml, while the average titer of AAPA virus from supernatantsof cells infected in the presence of MG132 was 2.2 × 10⁶ PFU/ml (Fig. 5A). Furthermore, unlike what was found for wild-typeVSV, the amounts of M protein present in both cell extracts andsupernatant samples either with or without MG132 were virtuallyidentical (Fig. 5B). Together, these results suggest that inhibitionof VSV release by MG132 is dependent on the presence of a functionalPY motif within the M protein.

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FIG. 5. Release of a VSV PY mutant is not blocked by MG132. (A) Titers of the AAPA mutant virus present in the supernatant of cells infected in the absence ( $-$ ) or presence (+) of MG132 (50 µM). Virus titers and standard deviations represent averages of three independent experiments. (B) Immunoprecipitation of radiolabeled VSV M protein from cell extracts (cells, lanes 2 and 3) and media (media, lanes 2 and 3) of cells infected in the absence ( $-$ ) or presence (+) of MG132 (50 µM). Mock-infected samples are shown in lane 1 in both sections.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The L domains of retroviruses, rhabdoviruses, and likely those of filoviruses are important for efficient budding and separationof progeny virions from infected cells. While their role in buddingis evident, the mechanism by which these L domains accomplishefficient virus-host separation remains unclear. Initial implicationsof the possible involvement of host proteins in virus buddingwere revealed by findings that viral L domains could mediate interactionswith cellular proteins (12-14, 39). Recently, a family of cellularproteins known as E3 ubiquitin ligases have been implicated inthe budding of retroviruses (34, 35, 37, 45, 49), filoviruses(13), and now rhabdoviruses (this report). One family member,Nedd4/Rsp5, is localized at the plasma membrane, plays a rolein ubiquitination and endocytosis, and possesses multiple typeI WW domains (3, 8, 9, 38, 42, 54, 55). Althoughwe had demonstrated previously that the L domains of VSV and RVcould mediate interactions with WW domains 2 and 3 of Nedd4/Rsp5(14), results described in this report have augmented the potentialsignificance of this virus-host interaction. For example, themouse Nedd4 gene was isolated from a cDNA library screen usingthe L domain of VSV as the bait, and the full-length VSV M proteininteracted both physically and functionally with full-length Rsp5in an in vitro ubiquitination assay. The wild-type VSV M proteinwas readily modified by the addition of ubiquitin; however, theprecise location(s) of ubiquitin addition within the M proteinhas yet to beidentified.

If ubiquitin or ubiquitin modification of the M protein were indeed important for virus budding, then decreasing the levelof free ubiquitin in the cell may adversely affect virus budding.Indeed, both VSV and RV release from infected cells was inhibitedby 10- to 20-fold in the presence of proteasome inhibitors, comparedto that in the absence of proteasome inhibitors. Control experimentsclearly demonstrated that inhibition of virus release was notsimply due to a global effect of the proteasome inhibitors onprotein synthesis. In general, these results are consistent withearlier findings that efficient release of retroviruses is inhibitedin the presence of proteasome inhibitors (37, 45, 49); however,the extent of inhibition of rhabdovirus release (10- to 20-fold)was consistently greater than that observed for retrovirus release(3- to 4-fold) (37, 45).

Results from experiments utilizing a VSV PY mutant demonstrated that the effect of proteasome inhibitors on virus releaseis associated with the presence of a functional L domain. Indeed,release of the VSV AAPA mutant was not significantly blocked inthe presence of MG132. These results are consistent with findingsreported previously for retrovirus budding in the presence ofproteasome inhibitors (45). Indeed, Schubert et al. demonstratedthat inhibition of HIV-1 budding by proteasome inhibitors wasdependent on both a functional L domain and a functional protease(45).

The fact that PY mutant forms of VSV (e.g., the AAPA mutant) can still bud from cells, albeit at significantly lower levelsthan wild-type VSV, indicates that additional viral sequencesare important for the budding process. One possibility is thatthere may be redundancy in the mechanism of virus budding at boththe virus and cellular levels. We have postulated previously thatadditional motifs that play a role in budding are likely presentwithin the M protein of VSV. For example, a PSAP motif, similarto the PTAPP motif within the Gag protein of HIV-1, is presentjust downstream of the PPPY motif in the VSV M protein. Similarly,the VP40 protein of Ebola virus contains overlapping PPxY andPTAPP motifs (13, 49). Although the M protein contains sufficientinformation to bud from cells independently of other viral proteins,it is certain that the G glycoprotein plays an important rolein VSV budding as well (30, 41, 48, 56). The functionalinteractions between M and G proteins of VSV remain of great interest,and deciphering these interactions will enhance our understandingof the molecular aspects of rhabdovirusbudding.

Many questions regarding the precise roles of ubiquitin and L domains in virus budding remain to be answered. For example,whether free ubiquitin or ubiquitin-modified forms of M proteinexist in VSV virions and in VSV-infected cells remains uncertain.Interestingly, ubiquitination of the RSV Gag protein has not beendetected thus far in virions; however, free ubiquitin has beendetected in both RSV and avian leukosis virus (40). Moreover,both free ubiquitin and ubiquitinated Gag molecules have beendetected in HIV-1 virions (32, 34, 35, 49). Ubiquitinmodification of these viral matrix proteins may function to (i)recruit additional cellular proteins (e.g., proteins involvedin endocytosis and/or exocytosis) required to facilitate virusbudding or (ii) target virus assembly and budding to specializedregions (e.g., lipid rafts) on the plasma membrane that are activeinvesicularization.

The fact that these three diverse families of RNA viruses may utilize a common approach to bud from cells is intriguing. Moreover,the ability to potentially inhibit release of these RNA virusesby targeting this late stage of budding remains an attractiveconcept. Further analysis of these potential virus-host interactionsin vivo is necessary and will serve to expedite our understandingof the role of the ubiquitin-proteasome machinery in virusbudding.

	ACKNOWLEDGMENTS

We thank D. S. Lyles, J. Paragas, N. T. Wright, and K.-K. Conzelmann for reagents and/orcomments.

This work was supported in part by a Formula Fund Award from the USDA to R.N.H. and NIH grant R01 GM-53726 to M.A.W.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Pathobiology, School of Veterinary Medicine, University of Pennsylvania,3800 Spruce St., Philadelphia, PA 19104-6049. Phone: (215) 573-4485.Fax: (215) 898-7887. E-mail: rharty{at}vet.upenn.edu.

Present address: Department of Molecular Biology, Princeton University, Princeton, NJ08544.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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