Coronavirus Pseudoparticles Formed with Recombinant M and E Proteins Induce Alpha Interferon Synthesis by Leukocytes

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Journal of Virology, November 1998, p. 8636-8643, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Coronavirus Pseudoparticles Formed with Recombinant M and E Proteins Induce Alpha Interferon Synthesis by Leukocytes

Pierre Baudoux, Charles Carrat, Lydia Besnardeau, Bernard Charley, and Hubert Laude^*

Unité de Virologie Immunologie Moléculaires, INRA, 78350 Jouy-en-Josas, France

Received 15 April 1998/Accepted 21 July 1998

	ABSTRACT

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Transmissible gastroenteritis virus (TGEV), an enteric coronavirus of swine, is a potent inducer of alpha interferon (IFN- $alpha$ )both in vivo and in vitro. Incubation of peripheral blood mononuclearcells with noninfectious viral material such as inactivated virionsor fixed, infected cells leads to early and strong IFN- $alpha$ synthesis.Previous studies have shown that antibodies against the virusmembrane glycoprotein M blocked the IFN induction and that twoviruses with a mutated protein exhibited a decreased interferogenicactivity, thus arguing for a direct involvement of M protein inthis phenomenon. In this study, the IFN- $alpha$ -inducing activity ofrecombinant M protein expressed in the absence or presence ofother TGEV structural proteins was examined. Fixed cells coexpressingM together with at least the minor structural protein E were foundto induce IFN- $alpha$ almost as efficiently as TGEV-infected cells.Pseudoparticles resembling authentic virions were released inthe culture medium of cells coexpressing M and E proteins. Theinterferogenic activity of purified pseudoparticles was shownto be comparable to that of TGEV virions, thus establishing thatneither ribonucleoprotein nor spikes are required for IFN induction.The replacement of the externally exposed, N-terminal domain ofM with that of bovine coronavirus (BCV) led to the productionof chimeric particles with no major change in interferogenicity,although the structures of the TGEV and BCV ectodomains markedlydiffer. Moreover, BCV pseudoparticles also exhibited interferogenicactivity. Together these observations suggest that the abilityof coronavirus particles to induce IFN- $alpha$ is more likely to involvea specific, multimeric structure than a definite sequence motif.

	INTRODUCTION

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Transmissible gastroenteritis virus (TGEV), a highly enteropathogenic virus of swine, belongs to the Coronavirus genus, agroup of enveloped viruses with a large (about 30-kb), positive-strandedRNA molecule as a genome (14; reviewed in reference 29). Likethose of other coronaviruses, TGEV virions are built from threemajor proteins: the N protein (47 kDa), with which the genomicRNA is packaged, and two envelope glycoproteins, S (220 kDa) andM (29 to 36 kDa) (29). Trimers of S protein form the prominentcoronavirus spikes (12). M, the most abundant component of coronavirions,is a polytopic protein spanning the membrane bilayer three times(reviewed in reference 42). When synthesized in the absenceof other viral components, M protein tends to accumulate in theGolgi complex as detergent-insoluble, polymeric structures, presumablyas part of its retention mechanism (26, 27). A third, smalltransmembrane protein, designated E (formerly sM), has been foundto be present at a low copy number in TGEV virions (19), aswell as in infectious bronchitis virus (IBV) and mouse hepatitisvirus (MHV) (35, 51). Coronavirus assembly has been shownto take place at membranes of the intermediate compartment, betweenthe endoplasmic reticulum and the Golgi complex (25). Recently,substantial progress toward an understanding of the mechanismof assembly has been made, with the demonstration that coexpressionof the MHV M and E proteins leads to the formation and secretionof particles closely resembling authentic virions (6, 48).

In vivo, TGEV replication takes place primarily in the differentiated enterocytes covering the villi of the small intestine(reviewed in reference 15). An ectoenzyme abundantly expressedat the brush border, aminopeptidase N, has been shown to act asa receptor for virus entry into target cells (11). In infectedanimals, high titers of interferon (IFN) are detected at boththe local and systemic levels (28). The observed IFN activityis primarily alpha IFN (IFN- $alpha$ ), thus making enterocytes unlikelyto represent the major IFN-producing cells. Subsequent studieshave revealed that incubation of swine peripheral blood mononuclear(PBM) cells from naive animals with TGEV-infected, fixed culturesor purified virus, as well as in vivo injection of UV-inactivatedvirions, leads to a marked and early IFN- $alpha$ synthesis (8, 38).Together, these observations support the view that such an inductionpathway, involving nonreplicating viral elements, mainly accountsfor the strong IFN response observed in TGEV infection.

There is now substantial evidence that IFN- $alpha$ synthesis can be triggered by inert viral structures, indicating that replicationand/or gene expression is not required for efficient IFN inductionat least in certain categories of lymphoid cells. This kind ofIFN- $alpha$ -inducing activity has been reported for enveloped virusesbelonging to many different groups, including paramyxo-, orthomyxo-,lenti-, rhabdo-, corona-, and herpesviruses (reviewed in reference16). In vitro studies using virus-induced blood leukocyte preparationshave allowed the definition of the IFN- $alpha$ -secreting cells as asmall but highly productive leukocyte subpopulation, referredto as natural interferon-producing (NIP) cells, able to synthesizeIFN- $alpha$ after a brief contact with noninfectious viral structures(16). Studies performed with human and pig blood leukocyteshave shown that NIP cells are nonphagocytic, nonadherent cellsthat lack T, B, and natural killer cell lineage-specific markersbut express CD4 and major histocompatibility complex class IImolecules (36, 44, 47).

The stimulation of IFN synthesis is assumed to be determined by an interaction of the NIP cell surface with one or severalviral components, but a limited number of studies have been aimedat understanding the nature of these viral components. Based oninhibitory effects of relevant antibodies, viral glycoproteinssuch as human herpes simplex virus protein D, human immunodeficiencyvirus (HIV) type 1 gp120, Newcastle disease virus HN, and viralhemorrhagic septicemia virus G protein have been proposed to playa role in IFN induction (17, 23, 34, 41). In the caseof TGEV, two lines of evidence have pointed to a role of the membraneprotein M as the major inducing component. First, within a panelof antibodies directed to the TGEV structural proteins, only twoblocked IFN induction, with both of them recognizing the shortN-terminal ectodomain of M (8). Second, two of the epitopemutants selected toward the above antibodies exhibited a markedlydecreased interferogenic activity. The substitutions identifiedin both mutant M genes mapped within the ectodomain and impairedthe glycosylation of the protein, without affecting the virusinfectivity (32).

The use of recombinant expression is a straightforward approach in assessing any interferogenic activity of individual viralproteins. Recently, two viral proteins have been reported to induceIFN- $alpha$ production by lymphohematopoietic cells independently fromany other viral component. Isolated recombinant HIV gp120 proteinexhibited some interferogenic activity for human PBM cells (2,7). Cells expressing HN protein of human parainfluenza virustype 4A had an ability to induce IFN in mouse spleen cells (22).In contrast, our attempts at demonstrating interferogenic activityassociated with recombinant TGEV M protein, transiently or stablyexpressed in mammalian cells, consistently failed (3, 4).Similar negative results were obtained when TGEV virion-derivedenvelope proteins reconstituted into virosomes were used (39).An interesting possibility suggested by these results was thatinteraction of M protein with NIP cells would not be sufficientin itself to trigger IFN synthesis, because either the putativeinterferogenic determinant needs to be presented in a specificcontext (such as the lipid bilayer) or the interferogenicity issubordinated to a polymeric structure. In order to test this hypothesis,the incidence of the expression of other viral proteins upon IFN- $alpha$ induction by TGEV M was examined. It was found that coexpressionof M and E proteins allowed the formation of pseudoparticles whichexhibit an interferogenic activity similar to that of completevirions.

(Part of these data have been presented at the International Symposium on Coronaviruses and Arteriviruses, Segovia, Spain,May 1997.)

	MATERIALS AND METHODS

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Virus and antibodies. The Purdue-115 strain was used as a TGEV source and propagated in ST cells as previously described (31). The following monoclonalantibodies (MAbs) were used: 25.22 and 3.60, directed to the N-terminaland cytosolic regions of TGEV M, respectively (31, 32); C29,directed to the C-terminal region of TGEV E (19); 53.13 and5.1, specific for TGEV S and N proteins, respectively (31);and 27P22 as an anti-bovine coronavirus (BCV) E antibody (suppliedby J. F. Vautherot, Jouy-en-Josas, France).

PBM cells. Nonadherent porcine PBM cells were obtained from heparinized blood by Ficoll density centrifugation on MSL (density, 1.077g/ml; Eurobio, Paris, France) followed by adherent-cell depletionon tissue culture flasks as described previously (36). PBM cellswere suspended in RPMI 1640 medium supplemented with 10% fetalcalf serum and antibiotics for IFN- $alpha$ induction assays.

IFN- $alpha$ induction. PBM cells were induced to produce IFN- $alpha$ by overnight incubation at 37°C with TGEV in 96-well microplates. Nonadherent cellswere incubated at a final concentration of 8 × 10⁶ cells per ml in a total volume of 0.2 ml with TGEV or pseudoparticlesat various dilutions, as shown in Results. In some of the experiments,PBM cells (8 × 10⁶ cells per ml in a total volume of 0.5 ml) were incubated overnightin 24-well plates with infected or transfected cell monolayersfixed with 0.25% glutaraldehyde as described previously (8).Cell supernatants were collected and stored at $-$ 20°C before IFN- $alpha$ immunoassay.

IFN- $alpha$ immunoassay. A specific enzyme-linked immunosorbent assay (ELISA) for porcine IFN- $alpha$ was performed as previously described (10, 46)by using MAb K9 for coating and MAb F17 as a second antibody.In each assay, our internal standard of recombinant porcine IFN- $alpha$ was included.

M antigen quantification. M antigen associated with purified pseudoparticles and virions was quantified by an ELISA as follows. Serial threefold dilutionsin 0.1 M sodium carbonate-bicarbonate buffer (pH 9.6) were incubatedovernight in a 96-well plate (PROBIND); coated wells were saturatedin phosphate-buffered saline-0.05% Tween 20-3% bovine serum albuminfor 2h at 37°C and then incubated for 90 min at 37°C with MAb25.22, 3.60, or 51.13 (as a negative control for pseudoparticles)ascites fluid diluted 1/1,000 in the same buffer. After washing,the samples were incubated with anti-immunoglobulin G (heavy pluslight chains) rabbit antibodies conjugated with alkaline phosphatase(1 µg/ml; Biosys) for 1 h at 37°C, washed, and incubated for 15to 30 min with para-nitrophenyl phosphate (Sigma) diluted at 1mg/ml in 0.05 M sodium carbonate-bicarbonate-10 mM MgCl₂ buffer(pH 9.8). The reaction was stopped by addition of 0.1 M NaOH.The optical density was measured at 405 nm on a Titertek MultiscanMCC/340. M and S antigens associated with fixed cell monolayerswere quantified by the same procedure.

Plasmid construction. TGEV and BCV M and E homologous and chimeric genes have been cloned into plasmid vectors providing the bacteriophage T7 transcription-regulatorysequences. All ligation junctions and sequences of inserts generatedby PCR were confirmed by automated sequencing (Applied Biosystems373A). The oligonucleotide primers used are listed in Table 1.

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TABLE 1. Amplimers used

(i) M gene constructs. TGEV M cDNA was obtained by reverse transcription-PCR of total mRNA from TGEV-infected ST cells with primers 2190 and 2282and cloned between the HindIII and EcoRI sites of pcDNA1 (InvitrogenCorporation) to give plasmid pTM2. The BCV M gene was PCR amplifiedfrom p174 (45) with primers 66830 and 66841 and cloned intothe EcoRV site of pBluescript II SK( $-$ ) (Stratagene). The BTT chimera,which encodes TGEV N-proximal sequence fused with BCV N-distalsequence at the homologous stretch WNFS (see Fig. 5a), was constructedby insertion of PCR fragments between the NcoI and EcoRI sitesof pTM1 (provided by B. Moss). The fragments were obtained bytwo-step amplification of p174 and pTM2 with primers 66830-2373and 72916-2282, respectively, followed by amplification with primers66830 and 2282, respectively. The reciprocal chimera TBB, i.e.,encoding TGEV N-proximal sequence fused with BCV N-distal sequence,was obtained by cloning into the EcoRV site of pBluescript a PCRfragment obtained by the same strategy described above with primerpairs 3247-85138 and 85139-66831 followed by 3247 and 66831.

(ii) E gene constructs. The TGEV E gene was PCR amplified from pTG2.15 (37) with primers 2414 and 2030 and cloned between the BamHI and XbaI sitesof pcDNA1 to give plasmid pcsM. In this construct, Thr at position2 is replaced by Ala as a consequence of the optimization of theATG context. The BCV E gene was amplified from pT7T3NS3 (50)with primers 627 and 519 and cloned between the EcoRI and BamHIsites of pcDNA3 to give plasmid p3NS3. The bt chimera, specifyinga protein with TGEV N-terminal and BCV C-terminal sequences fusedat the homologous stretch KLC (see Fig. 5a), and the reciprocalchimera tb were constructed by use of an NsiI site present withinthe KLC stretch. For bt, PCR fragments amplified from p3NS3 withprimers 2119 and 85137 were cloned after BamHI-NsiI restrictioninto the corresponding sites of pcsM to give pc34. For tb, PCRfragments amplified from pT7T3NS3 with primers 85136 and 2119were cloned into the EcoRV site of pBluescript. After BamHI-NsiIrestriction, the insert was subcloned into the corresponding sitesof pTMsM, to give pTM43. This plasmid was subjected to EcoRI-BamHIdigestion and ligation to remove the T7 promoter issued from pT7T3NS3.

(iii) Other constructs. The TGEV N gene was cloned into pcDNA1 as an EcoRV fragment from pTG2.18 (37) to give the plasmid pcN. pZG35 was used toexpress the full-length TGEV S protein under control of the T7promoter (20).

Transfection, metabolic labeling, and immunoprecipitation. Confluent monolayers of RK13 cells were infected with vaccinia virus vTF7.3 (18) at a multiplicity of infection of 5. At1 h postinfection the cells were transfected with Lipofectaminecontaining the appropriate plasmids in Optimem as recommendedby the manufacturer (GibcoBRL). At 3 to 5 h after DNA transfection,the cells were metabolically labeled by using methionine-depletedmedium (GibcoBRL) containing 2% fetal calf serum and 100 µCi of[³⁵S]methionine-cysteine (Tran³⁵S-label; ICN Biomedicals) per ml. At 10 h postinfection the mediumwas collected. The cells were lysed with 1× immunoprecipitationbuffer (50 mM Tris [pH 8], 40 mM EDTA, 0.5% Na deoxycholate, 0.5%Nonidet P-40, 0.5 ml of aprotinin per liter), and the lysate wascentrifuged at 4°C for 10 min at 10,000 × g. Immunoprecipitationwas performed with MAbs and protein A, and the resulting sampleswere analyzed by reducing sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and autoradiography, as previouslydescribed (31).

Velocity sedimentation. Culture medium of vTF7.3-infected cells expressing M and E proteins or of TGEV-infected cells labeled from 5 to 10 h postinfectionwas cleared at 10,000 × g for 10 min and loaded on a linear 20to 45% sucrose gradient. After centrifugation for 4 h at 25,000rpm in a Beckman SW40 rotor at 4°C, 20 fractions were collectedfrom the bottom, diluted 1:1, and centrifuged for 15 min at 300,000× g. Pelleted material was analyzed by SDS-PAGE as described above.

Purification of pseudoparticles. The starting material was produced from five 162-cm² flasks (Costar) of RK13 cells coexpressing the TGEV M and E genes. Eachmonolayer was infected with vTF7.3 at a multiplicity of infectionof 3 and then transfected with 10 ml of a 50-ml mixture containing40 and 120 µg of pTMM2 and pcsM plasmid DNAs, respectively, and1.2 ml of Lipofectin in Optimem. After 5 h, the monolayers wererinsed and maintained in Eagle minimal essential medium plus 10%fetal calf serum. The culture media were collected at 24 h postinfectionand processed as described for TGEV virions (31). The resultingconcentrated material was loaded onto two 20 to 45% sucrose gradientsand centrifuged for 3.30 h in an SW27 rotor. Pseudoparticle materialwas visible as a discrete, opalescent band which was collecteddirectly.

Electron microscopy. Formvar-carbon-coated grids were put in contact with a purified pseudoparticle suspension for 2 min, rinsed with phosphate-bufferedsaline plus 2% bovine serum albumin, and incubated for 30 minwith anti-TGEV M antibody 25.22 and then with protein G coupledto 10-nm-diameter gold particles (British Biocell International).Grids were viewed on a Philips EM12 electron microscope afterstaining with 2% phosphotungstic acid (pH 6.8).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

IFN induction by cells coexpressing TGEV M and E proteins. The vaccinia virus-T7-driven system was used to express the M protein alone or together with one or several of the other structuralproteins, including the minor structural protein E. After fixation,the cell monolayers were incubated with swine PBM cells, and theIFN activity present in the culture medium was quantified (Fig.1). As a striking result, cotransfection of M and E genes wasfound to be an absolute requirement for IFN induction. The levelof IFN production was higher than 10³ IU/ml, a titer which is not far from that observed when TGEV-infected,fixed cell cultures are used as an inducer in the same assay.The IFN induction was parallel to expression of M antigen at thesurface of the fixed cells, as determined by an ELISA test (datanot shown). This is consistent with the notion that accessibilityof M to PBM cells is a prerequisite for IFN induction. In addition,IFN induction was found not to be enhanced by the additional expressionof the virion proteins S and/or N. Both proteins were found tobe readily detectable in cultures cotransfected with the fourstructural genes, based on ELISA and indirect immunofluorescencetests. From these results, it was concluded that the coexpressionof M and E was both necessary and sufficient to induce IFN synthesis.This phenomenon appears to be independent of the cell context,as the same conclusion was reached when Cos7 or ST cells wereused for coexpression (data not shown) instead of RK13 cells asdone for Fig. 1.

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FIG. 1. Induction of IFN- $alpha$ by cell cultures expressing TGEV structural proteins. Vaccinia virus vT7-3-infected RK13 cells were transfected with Lipofectamine containing one or a combination of plasmids, each containing one of the TGEV genes, as indicated. The monolayers were fixed with 0.25% glutaraldehyde at 10 h postinfection and then incubated overnight with PBM cells (10⁷/ml) for IFN induction. TGEV- or mock-infected ST cell monolayers were processed in the same way for comparison. The interferon titer in the maintenance medium was determined by an ELISA test specific for IFN- $alpha$ .

TGEV pseudoparticles are released from cells coexpressing M and E. During the course of these studies, it was reported that the coexpression of MHV M and E proteins leads to the assembly andsecretion of particles closely resembling authentic coronavirions(6, 48). Accordingly, a possible explanation of the above-mentionedobservation was that the formation of similar viral structureswas a crucial parameter for TGEV M-mediated induction of IFN.The following experiments were performed in order to formallydemonstrate that formation and release of pseudoparticles alsooccurred in TGEV M- and E-expressing cells.

First, the material present in the medium from radioisotopically labeled, cotransfected or infected cultures was analyzedby ultracentrifugation in sucrose gradients. As shown in Fig.2, M protein material sedimented as a discrete peak, with a velocityclose to but lower than that of TGEV virions. No E protein couldbe detected in this experiment, presumably because it was incorporatedat a low ratio in the pseudoparticles, similar to that found forTGEV and MHV virions (19, 51).

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FIG. 2. Velocity centrifugation analysis of M protein material released from cells coexpressing TGEV M and E genes. The culture medium from vT7-3-infected, transfected, and labeled RK13 cells was centrifuged on a 20 to 45% linear sucrose gradient. The material present in each fraction was pelleted and analyzed directly by SDS-12% PAGE and autoradiography. The position (top of the peak) of labeled TGEV virions sedimented in a parallel gradient is shown by an open triangle. The sucrose concentrations in the fractions corresponding to the sedimentation peaks of pseudoparticles and virions, respectively, are shown (arrow).

Second, in an attempt to visualize the recombinant pseudoparticles, extracellular material derived from coexpressing cultureswas purified by sucrose gradient centrifugation and analyzed byelectron microscopy after immunogold labeling (Fig. 3). Negativestaining revealed a population of relatively homogeneous, sphericalparticles, the diameter of which was estimated to be 110 ± 10nm (n = 30), very similar to that determined for TGEV virions(spikes excluded). Thus, the data overall confirmed those obtainedfor MHV pseudovirions (48).

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FIG. 3. Electron microscopy of TGEV pseudoparticles. Particles secreted from RK13 cells coexpressing the M and E genes were purified by a procedure similar to that used for TGEV virions (see Materials and Methods). Particles were viewed after immunogold labeling with an anti-M ectodomain antibody and negative staining. The insert shows two pseudoparticles at a twofold-higher magnification.

TGEV pseudoparticles exhibit interferogenic activity. Experiments were next performed to learn whether material released in the medium from cultures cosynthesizing M and E throughvaccinia virus-T7 expression exhibited interferogenic activity.A substantial, dose-dependent IFN-inducing activity was foundto be associated with sedimentable extracellular material collectedafter pelleting through a glycerol cushion (data not shown). Importantly,no interferogenic material was released from cultures expressingM protein alone. A key issue was whether the specific interferogenicactivity of the recombinant particles compared to that of authenticTGEV virions. To address this, the contents of M antigen in sucrosegradient-purified preparations of recombinant pseudoparticlesand virions were determined by ELISA, and then dilutions of eithermaterial giving approximately the same signal were allowed toincubate with PBM cells. These experiments showed that the interferogenicactivity (i) persisted after purification of the pseudoparticles;(ii) was comparable for two batches produced and purified independently;(iii) was close to that of virions, i.e., about fivefold lessaccording to the data shown in Fig. 4, which were obtained withthe purified batch having the highest M antigen concentration;and (iv) was inhibited by an antibody directed to the N-terminalectodomain of the M protein to the same extent as for TGEV virions.

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FIG. 4. IFN- $alpha$ -inducing activity of recombinant pseudoparticles and TGEV virions. Purified recombinant particles and virions were obtained as described in Materials and Methods. Based on the results of an ELISA, the suspensions were adjusted to have approximately the same M antigen content and then incubated with PBM cells at the indicated dilutions. The blocking effect of anti-M MAb 25.22 on IFN induction is shown on the right. The ratio of virions to PBM cells was estimated to be 100 ng per 2 × 10⁵ cells at the 1/100 dilution.

IFN induction by chimeric TGEV-BCV pseudoparticles. The possibility of generating fully interferogenic particles by transient expression of two cloned viral genes made it temptingto use a genetic approach in an attempt to identify the moleculardeterminant(s) implicated in this phenomenon. To this end, itwas decided to generate chimeric particles through the use ofthe BCV E and M genes, which were previously cloned in the laboratory(45, 50). A first series of experiments were designed withthe aim of answering more specifically two questions: (i) whetherapart from its apparent morphogenic role, the minor componentE protein plays any role in the interferogenicity and (ii) whetherthe latter activity would be altered by a change in the M ectodomain,assuming that this is the main region of the protein interactingwith the IFN-producing cells.

The structures of the relevant constructs and the particle release results obtained are presented in Fig. 5. ExtracellularM material was readily detected in the culture medium of cellscoexpressing homologous (TGEV or BCV) M and E proteins, whereasvery little or no release was observed when either M-E heterologousconstructs or M-half-chimeric E constructs (tb and bt) were coexpressed(Fig. 5b). In contrast, the M chimera called BTT, in which theTGEV M ectodomain was replaced by that of BCV, was found to allowefficient particle formation (Fig. 5c). Furthermore, this BTTchimera appeared to lead to pseudoparticle formation with eachof the four E gene constructs. This finding was unexpected inview of our unsuccessful attempts to obtain particle formationthrough the coexpression of eight different TGEV-BCV chimericM proteins (3), as shown here for the TBB chimera.

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FIG. 5. Production of pseudoparticles by coexpression of heterologous and/or chimeric M and E genes of TGEV and BCV viruses. (a) Alignments of the sequences of mature TGEV and BCV M proteins (T and B, respectively) and of TGEV and BCV E genes (t and b, respectively). The predicted transmembrane segments are underlined in the TGEV sequences. Identical amino acids are in uppercase letters. In boldface are shown two short homologous regions selected to fuse TGEV and BCV sequences in the chimeric M or E gene constructs used in these experiments. Sequence data are from references 33 (TGEV M), 30 (BCV M), 19 (TGEV E), and 1 (BCV E). (b and c) Various pairs of homologous and chimeric constructs were expressed through the vT7-3 expression system. Particle assembly and secretion were assessed by monitoring the release of soluble, radiolabeled M material in the culture medium of transfected cells. Sedimentable material was collected by centrifugation through a glycerol cushion and analyzed by SDS-12% PAGE and autoradiography. The E chimera designated bt corresponds to the BCV amino-half sequence fused with the TGEV carboxy-half sequence, and tb is the reciprocal construct. The M chimera designated TBB corresponds to the TGEV N-terminal ectodomain fused with the remaining part of BCV M sequence, and vice versa for the BTT chimera. TBB and BTT chimeric proteins were expressed at equivalent levels as judged by immunoprecipitation assays of lysates of transfected cells with MAbs 25.22 and 3.60, respectively. Numbers on the left of panel b are molecular weights in thousands.

Interestingly, when the BTT chimera was analyzed for IFN induction, it was found to promote IFN synthesis as efficiently asthe parental TGEV M protein when coexpressed with TGEV E protein(Fig. 6a). The BCV M-E pair also induced IFN efficiently. WhenBTT was coexpressed with BCV E (BTT plus b), a significant butlower IFN-inducing activity was observed, consistent with thefact that this pair allowed less efficient particle formationthan the BTT-t pair or homologous pairs (Fig. 5c). Strikingly,no IFN-inducing activity could be detected in any of the cultureswhich expressed a pair of constructs unable to promote particlerelease (Fig. 6a and data not shown). As shown above with purifiedpseudoparticles (Fig. 4), a marked inhibition of IFN inductionwas observed when an antibody specific for the TGEV M ectodomainwas added during incubation with PBM cells (Fig. 6b). However,as expected, no inhibition occurred in the case of chimeric pseudoparticlesproduced with the BTT construct, which carries the BCV M ectodomain.

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FIG. 6. Induction of IFN- $alpha$ by cell cultures producing homologous or chimeric pseudoparticles of TGEV and BCV. The experiments were performed as described in the legend to Fig. 1. The coexpressed genes are indicated as uppercase letters on the x axis for M constructs and by lowercase letters for E constructs. For panel b, an antibody specific for the ectodomain of TGEV M protein was added in the culture medium during the incubation with PBM cells.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

As a main achievement, this study demonstrated that recombinant TGEV pseudoparticles, lacking spikes and ribonucleoprotein,can substitute for authentic virions to trigger efficient IFN- $alpha$ synthesis by swine leukocytes. It also revealed that BCV pseudoparticlesexhibit basically this same property, thus shedding new insightsinto the possible nature of the viral structure responsible forthis intriguing biological feature. Finally, based on attemptsat generating chimeric TGEV-BCV pseudoparticles, it was indicatedthat the formation of coronavirus particles involves highly specific,possibly multiple interactions.

The pseudoparticles were generated through the coexpression of the major virion component, i.e., the membrane M glycoprotein,and the minor, small membrane protein E (formerly called sM) andwere found to be the same size as TGEV virions. This observationconfirms that the notion of nucleocapsid-independent assembly,first described for the murine coronavirus MHV (6, 24, 48),extends to TGEV, which is representative of a distinct geneticsubset. The E protein-mediated release of M material has alsobeen observed with BCV (this study) and feline infectious peritonitisvirus (49), two viruses closely related to MHV and TGEV, respectively.It thus can be postulated that such a mechanism, in which theM and E proteins act as necessary and sufficient partners forbudding, is a general feature of coronaviruses, although thisremains to be formally established for IBV, which belongs to athird genetic group.

The induction of leukocytic IFN- $alpha$ by recombinant TGEV pseudoparticles essentially recapitulates the characteristics previouslyestablished for authentic virions. (i) The specific interferogenicactivity of purified pseudoparticles, estimated on the basis ofthe M protein content, closely approached that of TGEV virions.The small difference observed (Fig. 4) may be irrelevant, sincepseudoparticles and virions were produced in two different cellsystems. (ii) Antibodies directed to the M ectodomain were foundto prevent the IFN induction, as shown to be the case for TGEVvirions. (iii) Coexpression of the S protein had no discernibleeffect on IFN stimulation by pseudoparticle-producing cultures.This finding is in agreement with our earlier observations thatantibodies directed to either the S protein or its cellular receptorAPN had no effect on IFN induction by TGEV-infected cells or virions(8, 39). In the future, it might be of interest to see whetherrecombinant pseudoparticles made of unglycosylated M exhibit areduced interferogenic activity, as previously demonstrated forTGEV mutant viruses encoding M protein with an altered glycosylationsite (32). It would also be worth examining the interferogenicactivity of TGEV pseudoparticles toward PBM cells from differentanimal species, in order to compare the resulting cell spectrumwith that of virions, as it has been previously shown that IFN- $alpha$ induction by TGEV was not restricted to PBM cells from the swinespecies (8).

An important finding of this study was that the ability to induce strong IFN- $alpha$ synthesis by PBM cells is not a trait uniqueto TGEV pseudoparticles, as BCV recombinant particles were foundto exhibit basically the same property. This observation raisesthe question of whether the two viruses have a common interferogenicdeterminant. Stimulation of IFN synthesis must imply a physicalinteraction between pseudoparticle determinants and a subpopulationof PBM cells, the so-called NIP cells (see the introduction).The N-terminal ectodomain of the M molecule is stoichiometricallythe most abundant viral constituent exposed at the outer faceof the pseudoparticles, and this region was considered in ourearlier studies as a likely candidate for mediating such an interaction(32). It should be pointed out, however, that the N-terminalectodomains of TGEV and BCV differ notably in size and amino acidcomposition (Fig. 5a). The M ectodomain of TGEV potentially hasa more complex structure than that of BCV and, of possible relevance,is associated with a functional signal peptide, in contrast tothe case for most coronaviruses (33). Moreover, the carbohydratemoiety of M, previously shown to play a role in IFN inductionby TGEV (9, 32), differs between the two viruses: N and Oglycosylation for TGEV and BCV, respectively (13, 30). Inaddition, it was established during this study that a TGEV recombinantparticle, in which the ectodomain of M protein was replaced bythat of BCV, was as interferogenic as the homologous pseudoparticles.Together, these findings raise the possibility that the N ectodomainitself may not be the sole or the major determinant of the interferogenicactivity. It cannot be excluded, however, that TGEV and BCV particlesmay interact with different subpopulations of IFN-producing cells.Addressing this issue relies on the progress of ongoing studieson the identification and isolation of the NIP cells.

As an extension of the present study, we have examined whether the ability to induce IFN- $alpha$ is a general, so-far-unrecognizedfeature of coronaviral particles. As reported elsewhere, all ofthe eight viruses tested so far, including IBV, proved to be potentinducers for swine PBM cells, irrespective of their natural hostspecificity (5). Inspection of the reported M polypeptide sequencesfailed to reveal any conserved, contiguous sequence motif whichcould account for this function. Based on the accepted topologyof the M protein in the lipid membrane (42, 43), three regionsmight contain a determinant accessible to the effector cells.Both the N-terminal ectodomain and the short junction betweenthe transmembrane segments 2 and 3 are widely divergent amongthe three coronavirus groups. The third region includes a C-terminaldomain which would become externally exposed, assuming that someM virion-associated molecules comprise a fourth transmembranesegment, as was recently proposed for TGEV (40). Within thisregion, a 5-amino-acid stretch (YVKSK) is overall well conserved,except in IBV. In this respect, an antibody directed to the TGEVM endodomain failed to prevent IFN induction (8, 32). Finally,an alignment of the E protein sequences (19) did not revealany obvious candidate consensus motif either. Accordingly, itseems more plausible that the signal for IFN induction relieson a common structural feature than that it relies on a specificamino acid sequence motif.

In this study, we attempted to generate chimeric TGEV-BCV pseudoparticles as a possible approach to delineate an interferogenicdeterminant. Together, the results led us to conclude that a homologous,direct or indirect, interaction between the M and E proteins isrequired for efficient assembly, at least in the absence of otherviral components. No particle formation could be observed throughthe expression of TGEV M along with BCV E and vice versa. Restorationof particle formation through the coexpression of various combinationsof M and E chimeric constructs was subsequently attempted. Theseexperiments, the details of which will be reported in a separatepaper, proved to be generally unsuccessful (3). At least twolevels of blockade can be envisioned: M-M interaction, which isknown to occur (27) and is an obvious prerequisite for particleformation, and M-E interaction. The observed incompatibility couldreflect a complex process, in which several domains of the M andE polypeptide chains would be implicated in stereospecific interactions.It should be pointed out that no direct protein-protein interactionbetween M and E has been seen yet. Comparative studies performedwith four coronaviruses failed to reveal noticeable differencesin their budding sites in infected cells (25). However, subtledifferences in the subcellular localization of the TGEV and BCVproteins could account, at least in part, for the lack of assemblyof chimeric particles. In this respect, the production of particlesby use of the chimeric construct BTT, encoding a TGEV M proteinin which the ectodomain was replaced by its BCV counterpart, isintriguing. Indeed, coexpression of BTT not only with TGEV E butalso with either of the half-chimeric E proteins (tb or bt) andeven BCV E protein allowed particle formation, as if the specificityof M-E interaction was, at least in part, abolished. Clearly,additional studies are needed to address these important issues.

The mechanism by which inert viral particles, either free or associated with the cell surface, commit leukocytes to synthesizeIFN- $alpha$ remains elusive. To date, most of the viral proteins recognizedas playing a role in the induction are actually glycoproteins.On this basis, an interaction via a lectin-like activity has beenproposed as a common and central event for triggering IFN production(21). In the case of TGEV, there is indeed substantial evidencethat the carbohydrate moiety attached to the M protein does contributeto the interferogenic activity. Removal of complex, Golgi-modifiedoligosaccharides but not of mannose-rich oligosaccharides by treatmentof purified virions with appropriate glycosidases was shown tomarkedly reduce, but not abolish, the IFN induction (9). Also,the notable decrease in IFN-inducing ability of two TGEV mutantswas correlated with amino acid changes in the ectodomain of theM protein, which either suppressed or impaired the N-linked glycosylation(32).

For several reasons, however, an alternative scenario should be considered, in which the carbohydrate chain is only one componentof the stimulus necessary for signal transduction. First, thereis both direct and indirect evidence against a role of the spikeS protein, a heavily glycosylated protein (34% carbohydrate) (13),in IFN induction (see above). Second, envelope protein-liposomemixtures prepared from purified virions repeatedly failed to induceIFN, despite the fact that these structures expressed both M andS representative epitopes; furthermore, such virosomes appearedto compete with TGEV for IFN induction (39). Third, all of ourattempts to stimulate IFN production by using nonlysed cells,intracellular membranes, or detergent-solubilized material fromcultures singly expressing TGEV M (reference 4 and this study)were unsuccessful. Conversely, IFN induction was observed eachtime that particle formation was observed.

In conclusion, our data lend support to the view that the IFN- $alpha$ -inducing activity of coronavirus M protein could rely uponits incorporation into a polymeric, specifically organized structure.Moreover, we suggest that such a notion might be relevant forviruses other than coronaviruses. Taking HIV as an example, itis striking that the ability of virions to trigger IFN- $alpha$ inductionin PBM cells is dramatically higher than that of soluble gp120protein (17). Densely arranged and ordered repetitive structuresare a hallmark of infectious agents, including viruses, and ithas been proposed that B cells can discriminate between harmlessand harmful nonself antigens according to pattern or antigen organization(52). Along the same lines, it can be speculated that the spatialorganization is one of the factors determining the ability ofNIP cells to differentiate between endogenous glycoproteins andnonself, virus-associated glycoproteins.

	ACKNOWLEDGMENTS

We thank Emmanuel Kut for technical support, Patrice Vende for DNA sequence confirmation, Stephan Chilmonczyk for assistancewith electron microscope experiments, Pascal Boireau for the plasmidscontaining the BCV M and E genes, Jean-François Vautherot foranti-BCV E protein MAbs, and Roger Morris for editing of the English.

	FOOTNOTES

^* Corresponding author. Mailing address: Unité de Virologie Immunologie Moléculaires, INRA, 78350 Jouy-en-Josas, France. Phone:33 1 01 34 65 26 13. Fax: 33 1 01 34 65 26 21. E-mail: laude{at}biotec.jouy.inra.fr.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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