Measles Virus Assembly within Membrane Rafts

doi:10.1128/JVI.74.21.9911-9915.2000

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Journal of Virology, November 2000, p. 9911-9915, Vol. 74, No. 21
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Measles Virus Assembly within Membrane Rafts

Séverine Vincent, Denis Gerlier,^* and Serge N. Manié

Immunité & Infections Virales, VPV, CNRS-UCBL UMR 5537, Faculté de Médecine Lyon RTH Laennec, 69372 Lyon Cedex 08, France

Received 29 February 2000/Accepted 10 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

During measles virus (MV) replication, approximately half of the internal M and N proteins, together with envelope H and Fglycoproteins, are selectively enriched in microdomains rich incholesterol and sphingolipids called membrane rafts. Rafts isolatedfrom MV-infected cells after cold Triton X-100 solubilizationand flotation in a sucrose gradient contain all MV componentsand are infectious. Furthermore, the H and F glycoproteins fromreleased virus are also partly in membrane rafts (S. N. Maniéet al., J. Virol. 74:305-311, 2000). When expressed alone, theM but not N protein shows a low partitioning (around 10%) intorafts; this distribution is unchanged when all of the internalproteins, M, N, P, and L, are coexpressed. After infection withMGV, a chimeric MV where both H and F proteins have been replacedby vesicular stomatitis virus G protein, both the M and N proteinswere found enriched in membrane rafts, whereas the G protein wasnot. These data suggest that assembly of internal MV proteinsinto rafts requires the presence of the MV genome. The F but notH glycoprotein has the intrinsic ability to be localized in rafts.When coexpressed with F, the H glycoprotein is dragged into therafts. This is not observed following coexpression of either theM or N protein. We propose a model for MV assembly into membranerafts where the virus envelope and the ribonucleoparticle colocalizeandassociate.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The replication cycle of the morbillivirus measles virus (MV) occurs within the cytosol of target cells. After transcribingthe genome to allow virus protein synthesis, the MV RNA-polymeraseL associated with its cofactor, the phosphoprotein P, replicatesthe genome, which is simultaneously encapsidated by the nucleoproteinN (14). Together with the L and P proteins, the RNA-proteincomplex is assembled into the replication unit or ribonucleoparticle(RNP). The last step of MV assembly involves the wrapping of theRNP into an envelope derived from cell membrane regions enrichedin the cytosolic M protein and two integral membrane glycoproteins,the hemagglutinin (H) and fusion (F) proteins (14). A currentmodel favors an organizer role for the M protein, which linesthe inner surface of the virus envelope. The M protein, whichcan interact with the cytoplasmic tail of the F protein (28),appears to act by concentrating the F and H proteins, as wellas the RNP, at the site of virus assembly (3). Ultrastructuralstudies have shown that the final MV assembly likely occurs atthe plasma membrane (6, 21). Alteration of MV assembly, includingabrogation of M protein function, is likely responsible for arare persistent infection of the central nervous system by MV,subacute sclerosis panencephalitis (3).

Recently, we proposed that specific regions of the plasma membrane called rafts may provide a site for the assembly of MV(19). Rafts are cholesterol- and glycosphingolipid-rich microdomainsoriginally characterized by their insolubility at 4°C in nonionicdetergent such as Triton X-100 (2). Recent reports favor theconcept of rafts in living cells (9, 30). Glycosphingolipidshave the properties of self-association and association with cholesterol(12) to constitute liquid-ordered membrane domains which areresistant to cold solubilization by nonionic detergents (1,25). Such nonsolubilized membranes can be isolated from low-densityfractions after flotation in a sucrose gradient (2). Some proteins,such as those anchored by a glycosylphosphatidylinositol moiety,are resident in rafts (2). Membrane rafts from MV-infectedhuman cells are enriched in MV structural proteins since theycontain 30 to 50% of the viral proteins and less than 5% of totalcell proteins (19). The mature cleaved form of the F glycoprotein(F1F2 disulfide-linked heterodimer) but not the uncleaved F0 precursorassociates with rafts (19), in agreement with the raft assemblyprocess from the Golgi (26). Furthermore, isolated rafts containall components required to create a functional virus, as revealedby their ability to infect cells. Finally, MV components frommembrane rafts are incorporated into released MV particles. Thiswork was undertaken to determine which MV component(s) can localizeand assemble intorafts.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells. Human epithelial (HeLa) cells were grown in Dulbecco's modified Eagle's medium supplemented with 6% heat-inactivated fetalcalf serum, 10 mM HEPES, 2 mM glutamine, and 10 µg of gentamicinper ml at 37°C in the presence of 7% CO₂.

Viruses. The Edmonston strain of MV (23) and the chimeric virus MGV, where the reading frames of MV envelope glycoproteins H andF (MV-H and -F) were replaced by a single reading frame encodingthe vesicular stomatitis virus G glycoprotein (VSV-G) (28),were amplified on Vero cells. The recombinant vaccinia virusesvvH, vvF, vvHF, vvN, vvNF (31), vvNP, vvNPL (15), and vvM(32) were amplified on BHK-21 cells. After one cycle of freezing/thawingof infected cells, clarified supernatants were collected and usedas virusstocks.

Infections. After incubation overnight, HeLa cells were infected at the indicated MOI (multiplicity of infection). After 1 h at 37°C,the cells were washed once with fresh medium and incubated at37°C in the presence or absence of the fusion-inhibitory peptideZ-D-Phe-L-Phe-Gly (24) at 20 µg/ml. The cells were collected24 h after MV infection and 7 days after MGV infection in orderto obtain virus protein expression in most cells at the onsetof massive virus release. Infection or coinfection with recombinantvaccinia virus lasted 24 h prior to membrane raftanalysis.

Antibodies. The following antibodies were used: rabbit anti-MV-F cytoplasmic tail, produced as reported by Cathomen et al. (4); anti-MV-H,BH195 (8); anti-MV-N, C125 (10); anti-MV-P, a mouse anti-MVserum; anti-MV-M (Chemicon, Temecula, Calif.); anti-CD55, 12A12(17); anti-CD71 (Zymed Laboratories, San Francisco, Calif.);and anti-VSV-G, P5D4 (Sigma, St. Louis, Mo.).

Isolation of membrane rafts after Triton X-100 extraction at 4°C and flotation on sucrose gradients. Infected HeLa cells (3 × 10⁶), washed in ice-cold phosphate-buffered saline and harvested in phosphate-buffered saline-EDTA,were lysed on ice for 20 min in TNE (25 mM Tris-HCl [pH 7.4],150 mM NaCl, 5 mM EDTA) containing 0.5% Triton X-100 and a cocktailof protease inhibitors (Complete; Boehringer Mannheim). The celllysate volume was made up to 800 µl with TNE and sucrose 60% (wt/wt)to obtain a 45% sucrose concentration in a 6-ml centrifuge tube.The lysate was sequentially overlaid with 2.5 ml of 30% sucroseand 1 ml of 2.5% sucrose in TNE. The gradient was centrifugedat 200,000 × g for 16 h in an SW50.1 rotor (Beckman) and fractionatedfrom the top of the tube in eight fractions. The membrane raftsare resistant to solubilization by Triton X-100 at 4°C, and theirflotation allows their recovery from the low-density fractions(fractions 2, 3, and 4) of the discontinuous sucrosegradient.

Western blot analysis. An aliquot of each fraction was used for immunoblotting. Proteins were separated by sodium dodecyl sulfate-polyacrylamidegel electrophoresis and then transferred onto a polyvinylidenedifluoride membrane. Membranes were saturated with 5% nonfat driedmilk in TBS-T (20 mM Tris-HCl [pH 7.6], 150 mM NaCl, 0.1% Tween20) and incubated for 1 h with specific antibodies in TBS-T-1%milk. Immunoreactive bands were visualized by using secondaryhorseradish peroxidase-conjugated antibodies (Promega, Madison,Wis.) and enhanced chemiluminescence (Boehringer Mannheim). Quantificationof the autoradiograms was performed after scanning, using theImageQuant software (MolecularDynamics).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

The internal MV proteins associate with rafts only when coexpressed with the MV genome. Membrane rafts were isolated from MV-infected HeLa cells after cold solubilization with 0.5% Triton X-100 and flotation ina sucrose gradient. The low-density fractions 2, 3, and 4 containedthe membrane rafts, as shown by the predominant localization ofthe glycolipid-anchored CD55, a protein resident of rafts (Fig.1A). A significant proportion of the MV proteins (~16% of H, ~59%of F, ~42% of N, and ~45% of M) was found to be associated withthe rafts (Fig. 1A; Table 1). To verify the ability of internalMV proteins to localize within the rafts in the absence of theenvelope H and F transmembrane proteins as previously observedin another cell line (19), the HeLa cells were infected withMGV (see Materials and Methods) (2). Similar proportions ofMV-N and -M (~63 and 44%, respectively; Table 1) were found tobe associated with rafts, which contain ~95% of the CD55 raftmarker but less than 4% of VSV-G (Fig. 1B). To evaluate the intrinsicability of internal MV proteins to localize into the rafts, theM and N proteins were expressed alone or in association with otherMV internal proteins after infection with recombinant vacciniavirus. When expressed alone, only trace amounts of the N protein(~2%) and a low but constant amount of M (~20%) could associatewith the rafts (Fig. 1C; Table 1). The coexpression of N withP, N with P and L, or the four MV internal proteins N, P, L, andM did not result in any change in the distribution of N or M withinthe sucrose gradients. Taken together, these results indicatethat the M but not the N protein has an intrinsic, albeit low,ability to associate with the membrane rafts and that a majorredistribution of the M and N proteins into rafts requires thepresence of the MV genome.

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FIG. 1. Only coexpression of the MV genome allows the N and M proteins to localize into membrane rafts. HeLa cells were infected for 2 days at an MOI of 1 with MV tag (A), for 7 days with MGV (MOI of 2) (B), or for 24 h with recombinant vaccinia virus (MOI of 5) encoding one, two, three, or four of the MV internal proteins (C). Cells were then lysed with 0.5% Triton X-100 at 4°C, and the membrane rafts were separated by flotation on a discontinuous sucrose gradient. Immunoblot analyses of MV proteins from each fraction of the gradient (fraction 1 represents the top of the gradient) were performed with specific antibodies. The distributions of CD55, a resident of rafts, and of G protein, which is not located in rafts, are shown as controls.

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TABLE 1. Cumulative data from several experiments showing the distribution of MV proteins within membrane rafts

MV-F can drag MV-H into rafts. The ability of the envelope glycoproteins to associate with membrane rafts was then investigated. When expressed alone usingrecombinant vaccinia virus, ~47% of the F1 protein and ~1% ofthe H protein were found to localize with the rafts characterizedby their high CD55 contents. As previously reported (33), theCD71 molecule did not cosediment with rafts (Fig. 2A and B). However,when coexpressed with the F protein, ~29% of the H protein wasfound to associate with the raft fractions (Fig. 2C). This increasein raft localization of the H protein was specific since the CD71molecule remained nonassociated with the rafts. Thus, MV-F hasthe intrinsic ability to associate with the membrane rafts andcan drag into them the H glycoprotein as well.

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FIG. 2. MV-F drags MV-H into membrane rafts. HeLa cells were infected for 24 h with recombinant vaccinia virus (MOI of 5) encoding MV-F (A), MV-H (B), or both (C). Cells were then subjected to extraction by Triton X-100 at 4°C and flotation. The distribution in the gradient of MV proteins together with CD55 and CD71 as control proteins was assayed by Western blotting.

Inability of MV-F to drag internal MV proteins. Coexpression of the envelope F glycoprotein with the internal M or N protein after infection with recombinant vvNF or bothvvM and vvF did not result in any change in the distribution ofthe M and N proteins throughout the sucrose gradient (Fig. 3A).Indeed, although ~40% of F1 colocalized with most of the CD55in the light fractions, only trace amounts of the N and ~10% ofthe M protein were found associated with these fractions, as observedin the absence of the F protein.

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FIG. 3. Neither MV-F (A) nor the MV RNP (B) can drag into membrane rafts the internal MV proteins (A) and MV-H (B). (A) HeLa cells infected with the recombinant vaccinia viruses (MOI of 5) indicated at the left; (B) cells coinfected with MGV (MOI of 2) and with vaccinia virus encoding MV-H. Cells were analyzed as described for previous figures.

Inability of the MV RNP to drag H protein into rafts. Likewise, coexpression of the MV RNP with the H glycoprotein, after super infection of MGV-infected HeLa cells with vvH, didnot allow the H glycoprotein to significantly associate with therafts (Fig. 3B). Indeed, ~32% of the N and M proteins and onlytrace amounts of the G and H proteins cosedimented with ~82% oftheCD55.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

When MV-H, -F, -M, and -N were expressed alone using recombinant vaccinia virus, only the F and M proteins exhibited highand low, respectively, intrinsic abilities to localize into thecell membrane rafts. A possible interference of the vaccinia virusinfection in the distribution of MV proteins in rafts was excludedbecause (i) the distribution of MV proteins in infected cellsremained unchanged after coinfection with a vaccinia virus (unpublisheddata; see also the similar distributions of MV-M and -N afterinfection with MGV [Fig. 1B] and coinfection with vaccinia virus[Fig. 3B]) and (ii) similar results were obtained when these proteinswere transiently expressed using eukaryotic vectors(unpublished).

Coexpression of the RNP proteins N, P, and L did not result in a significant redistribution of the N protein into the rafts.This could be due neither to the lack of N polymerization, becausecoexpression of the N and P proteins spontaneously results inthe formation of nucleocapsid-like structures likely wrappingcellular RNAs (7, 27), nor to the use of recombinant vacciniavirus, because similar results were obtained for the 293-3-46cell line (23), which constitutively expresses both N and Pproteins (not shown). Likewise, an unbalanced proportion of N,P, and L proteins was unlikely, since the three proteins wereexpressed in proportion suitable for the transcription and replicationof an MV CAT-DI minigenome (reference 15 and data not shown).When the M protein was coexpressed with the N, P, and L proteins,the N protein did not redistribute to the rafts despite the knowninteraction of the RNP with the M protein (13, 29). Only thepresence of the MV genome resulted in the strong targeting ofboth M and N proteins into the membrane rafts. We propose thatonly the MV genome RNA could allow the formation of the RNP scaffoldfor wrapping into an M protein lattice. This lattice would inturn be more efficiently targeted to (or more stably associatedwith) the rafts than isolated Mproteins.

The F protein allows the H glycoprotein to associate with the membrane rafts in a proportion similar to that observed afterMV infection. This correlates with the known propensity of thesetwo components of the virus envelope to interact with each other.Indeed, the H and F proteins can be coimmunoprecipitated (18),and several observations argue for their association into a functionalcomplex allowing the fusion of the virus envelope with the targetcell membrane. (i) Mutant H and F proteins should be appropriatelypaired (5). (ii) The fusion helper function of H is ablatedby a single amino acid substitution at residue 98 (16). (iii)Some anti-H monoclonal antibodies inhibit the fusion step withoutinhibiting attachment of the H protein to the CD46 cellular receptor(11, 16).

The M protein can interact with the cytoplasmic tail of the F protein. Indeed, it is specifically recruited into the recombinantvirus MG/FV, where the H and F genes have been replaced by a geneencoding VSV-G fused to the cytoplasmic tail of MV-F, whereasthe M protein was excluded from the MGV particles (28). Theassociation of the M protein with the rafts is, however, not enhancedwhen M is coexpressed with the F protein. This suggests that astable interaction of the M protein with the F cytoplasmic tailrequires its association with the MV RNP and enhanced localizationinto the rafts. Likewise, the inability of the M-RNP complex todrag the H glycoprotein into the rafts indicates that the putativeinteraction of M with the cytoplasmic tail of H is too weak orabsent. While this report was under review, Naim et al. showedthat in MV-infected polarized human epithelial cells, F and Hglycoproteins are intrinsically targeted to the basolateral siteand that M protein reverts the transport of F and H glycoproteinsfrom the basolateral site to the apical cell surface, where MVbudding occurs (20). Since the later targeting is often associatedwith the interaction of sorting signals in the trans-Golgi networkwith membrane rafts (26), they postulated that the membranerafts could be involved in the apical sorting of MV nucleocapsidand glycoproteins. If this is true, one prediction derived fromtheir and our findings would be that the M protein expressed inthe absence of the RNP should not be appropriately targeted tothe apical site and/or able to redirect the F protein to the apicalsite.

Taken together, our data suggest that the membrane rafts can act as platforms for the assembly of MV prior to virus budding.We propose the following assembly model for MV (Fig. 4). The Fglycoprotein is spontaneously targeted to the rafts (step 1),and its ability to associate with its envelope partner, H, allowsthe localization of H-F complexes within the rafts (step 2). Whichof these two steps comes first will depend on the ability of Hand F proteins to interact early during their biosynthesis withinthe endoplasmic reticulum. Independently, the RNA genome and theN, P, and L proteins associate to form the RNP in the cytosol(step 3); this allows scaffolding of the M lattice and targetingof the M-RNP complex to the rafts owing to the discrete intrinsicpropensity of the M protein to associate with membrane rafts (step4). Through the interaction of the M lattice with the cytoplasmictail of the F protein, the M-RNP complex merges with the membraneenvelope H and F glycoproteins within the raft platform (step5). The envelope-RNP complex would now be ready for budding intomature MV particles. These steps do not necessarily occur sequentiallyand may be synchronized. Furthermore, this model is likely tobe oversimplified. The assembly process could involve at one stagethe coalescence of several membrane rafts, owing to their smallsize (<70 nm in diameter) determined on the plasma membrane ofviable cells (22, 30). The latest step of virus formationinto close vesicles is also not drawn because analysis of maturevirus particles has shown that they are made partly of nonraftmembranes (19), indicating that any budding trough membranerafts would be associated with capture of adjacent nonraft membranes.This model is now being tested to establish whether MV buds exclusivelythrough membrane rafts or also through a raft-independent pathway.

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FIG. 4. Assembly model for MV. The F glycoprotein is spontaneously targeted to the rafts (step 1) and drags the H protein into the rafts (step 2). Which of these two steps come first will depend on the ability of H and F proteins to interact early during their biosynthesis within the endoplasmic reticulum. Independently, the RNA genome and the N, P, and L proteins associate into the RNP in the cytosol (step 3). Interactions with the M protein enable the M-RNP complex to associate with the rafts (step 4). The interaction of the M lattice with the cytoplasmic tails of the F proteins allows merging of the M-RNP complex with the membrane envelope H and F glycoproteins within the raft platform (step 5). These steps do not necessarily occur sequentially and may be synchronized. Furthermore, this model is likely to be oversimplified; for example, it is not unlikely that the assembly process involves at one stage the coalescence of several membrane rafts (see text).

	ACKNOWLEDGMENTS

We thank R. Drillen, M. Billeter, H. Y. Naim, R. Cattaneo, E. Rubinstein, C. P. Muller, and F. Wild for providing useful reagents,P. Riou for help in performing CAT measurements, and D. Christiansenfor help in writing themanuscript.

This work was supported in part by grants from the ARC (SM, 9501) and the Ministère de l'Education Nationale, de la Rechercheet de la Technologie(PRFMMIP).

	FOOTNOTES

^* Corresponding author. Mailing address: Immunité & Infections Virales, VPV, CNRS-UCBL UMR 5537, Faculté de Médecine LyonRTH Laennec, 69372 Lyon Cedex 08, France. Phone: 33 4 78 77 8618. Fax: 33 4 78 77 87 54. E-mail: gerlier{at}laennec.univ-lyon1.fr.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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