RGD Tripeptide of Bluetongue Virus VP7 Protein Is Responsible for Core Attachment to Culicoides Cells

doi:10.1128/JVI.75.8.3937-3947.2001

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Journal of Virology, April 2001, p. 3937-3947, Vol. 75, No. 8
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.8.3937-3947.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

RGD Tripeptide of Bluetongue Virus VP7 Protein Is Responsible for Core Attachment to Culicoides Cells

Boon-Huan Tan,¹^,² Emma Nason,² Norbert Staeuber,¹^,² Wenrong Jiang,² Katherine Monastryrskaya,¹^,² and Polly Roy¹^,²^,³^,^*

Department of Biochemistry, University of Oxford, Oxford OX1 3QU,¹ and Institute of Virology & Environmental Microbiology, Oxford OX1 3SR,² United Kingdom, and Department of Medicine, University of Alabama at Birmingham, Birmingham, Alabama 35294³

Received 9 October 2000/Accepted 19 January 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Bluetongue virus (BTV) is an arthropod-borne virus transmitted by Culicoides species to vertebrate hosts. The double-capsidvirion is infectious for Culicoides vector and mammalian cells,while the inner core is infectious for only Culicoides-derivedcells. The recently determined crystal structure of the BTV corehas revealed an accessible RGD motif between amino acids 168 to170 of the outer core protein VP7, whose structure and positionwould be consistent with a role in cell entry. To delineate thebiological role of the RGD sequence within VP7, we have introducedpoint mutations in the RGD tripeptide and generated three recombinantbaculoviruses, each expressing a mutant derivative of VP7 (VP7-AGD,VP7-ADL, and VP7-AGQ). Each expressed mutant protein was purified,and the oligomeric nature and secondary structure of each wascompared with those of the wild-type (wt) VP7 molecule. Each mutantVP7 protein was used to generate empty core-like particles (CLPs)and were shown to be biochemically and morphologically identicalto those of wt CLPs. However, when mutant CLPs were used in anin vitro cell binding assay, each showed reduced binding to Culicoidescells compared to wt CLPs. Twelve monoclonal antibodies (MAbs)was generated using purified VP7 or CLPs as a source of antigenand were utilized for epitope mapping with available chimericVP7 molecules and the RGD mutants. Several MAbs bound to the RGDmotif on the core, as shown by immunogold labeling and cryoelectronmicroscopy. RGD-specific MAb H1.5, but not those directed to otherregions of the core, inhibited the binding activity of CLPs tothe Culicoides cell surface. Together, these data indicate thatthe RGD motif present on BTV VP7 is responsible for Culicoidescell bindingactivity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Orbiviruses (within the family Reoviridae), are vectored to vertebrate species by arthropods (e.g., gnats, mosquitoes andticks) and are able to replicate in both hosts. Bluetongue virus(BTV) is the prototype virus of the genus and is transmitted bygnats (Culicoides species), causing diseases of economic importancein ruminants in many parts of the world. Vector-virus interactionsplay a crucial role in vector-borne disease epidemiology. Thespread of Culicoides species from BTV-endemic to non-BTV (or relatedAfrican horsesickness virus, AHSV, and epizootic hemorrhagic diseasevirus EHDV, of deer) regions of the world in the past highlightsthe concern that these viruses are a threat to regions of theworld that are presently free fromthem.

The initiation of a virus infection involves virus binding to ligands on the cell surface prior to cell entry by a numberof mechanisms (depending on the virus). Like many other viruses,BTV appears to utilize a protein molecule(s) of mammalian cellsas a receptor (20); however, it is also possible that alternativereceptors may be utilized in different tissues and in differentspecies and as accessorymolecules.

BTV has a genome composed of 10 segments of double-stranded RNA packaged within a double icosahedral capsid. The outer capsidlayer, which is lost at an early stage of the infection process,is composed of two major structural proteins (VP2 and VP5). Theseproteins are involved in host cell attachment and penetrationduring the initial stages of infection (22). After entry intothe cells, the virus is uncoated (by removal of VP2 and VP5) toyield a transcriptionally active core particle which is composedof two major proteins (VP7 and VP3) and three minor proteins (VP1,VP2, and VP3) in addition to the double-stranded RNA genome (28,55, 56). Since BTV and other orbiviruses are transmitted betweentheir mammalian hosts by the bite of insect vectors, the virusesmust remain infectious in the insect gut, an environment whichcan remove the BTV outer layers. This implies that BTV particles,either lacking the complete outer capsid proteins or with modifiedouter capsid proteins, are infectious for the insect vector. Indeed,Mertens and coworkers have demonstrated that BTV cores are highlyinfectious for the Culicoides vector and Culicoides-derived cellculture (KC cells) (42-44) and that the specific infectivity ofin vitro-generated cores for the KC cells was directly comparableto that of the intact virus particles. Cores were similarly infectiouswhen oral infectivity studies were carried out using Culicoidesspecies. The high level of core-associated infectivity for KCcells suggests that the initial stages of core-cell interactionand entry use an alternate entry mechanism to that used by completeparticles.

The outermost BTV core protein, VP7, is the most accessible protein of the BTV core and suggests that it may participate invector cell entry (67). VP7 has an arginine-glycine-aspartate(RGD) tripeptide motif present at amino acid residues 168 to 170,one of the ligand sites recognized by host proteins that belongto the integrin family, such as fibronectin, vitronectin, andfibrinogen (29, 57, 58). From X-ray crystallographic structures,the RGD motif in BTV VP7 is located on the upper domain of thetwo domain molecule (1, 19) and appears to be accessibleon the surface. The RGD motif has a conformation similar to thatseen in the RGD motif of the VP1 protein of foot-and-mouth diseasevirus (FMDV) and $gamma$ -crystallin, which attaches to $alpha$ _V $beta$ ₃ integrin(6, 19, 20, 32, 38, 50, 51, 66). It is plausible,therefore, that RGD-integrin binding is an initial step of BTVcore attachment to insectcells.

In this study we have evaluated the role of the VP7 RGD sequence in cell attachment activity by taking advantage of an establishedbiological assay system which allows synthesis and purificationof high-yield recombinant core-like particles (CLPs) from Sf9insect cells (17). Not only are the CLPs composed of VP7 andVP3 antigenically equivalent to the BTV core but also both havesimilar three-dimensional (3D) structures when analyzed by cryoelectronmicroscopy (cryo-EM) (23-25). Thus, CLPs mimic the authentic coreand could be used as a surrogate of authentic cores in cell bindingstudies. We have introduced point mutations within the RGD tripeptideof the VP7 protein to generate VP7 with an altered RGD motif.Three such RGD-targeted VP7 mutants were expressed using the baculovirusexpression system, and their antigenic and biochemical propertieswere characterized. Each mutant derivative also assembled intoCLPs in the presence of the VP3 protein, implying that the RGDsite is accessible and is not involved in protein-protein interactionsduring core assembly. In addition, a panel of 12 monoclonal antibodies(MAbs) was raised against the VP7 protein and characterized. Anantigenic site corresponding to the RGD sequence of VP7 was subsequentlymapped by reacting the antibodies with the VP7 mutants in enzyme-linkedimmunosorbent assay (ELISA) based tests and by using immunogoldlabeling of CLPs. The general location of antibody binding wasconfirmed by cryo-EM studies. When these mutant CLPs were assessedfor their binding activities in Culicoides cells, each preparationshowed a decreased level of binding in comparison to the wild-type(wt) CLPs. Together, the data presented here demonstrate thatthe VP7 RGD motif is involved in the binding of the BTV core intoCulicoidescells.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses and cells. Spodoptera frugiperda (Sf9) cells were grown in suspension or monolayer cultures at 28°C in TC100 medium supplemented with10% fetal calf serum. Derivatives of Autographa californica nuclearpolyhedrosis virus containing the wt BTV-10 VP7 or BTV-17 VP3gene (Ac10BTV7 and Ac17BTV3) and the BTV-10 VP7 mutants were plaquepurified and propagated as described previously (17). The KCcell line, derived from the embryos of AK colony insects (63),was kindly provided by Sally Wechsler, US Department of AgricultureCenter, Laramie, Wyo., and were grown at 28°C in Schneider's medium(Sigma) supplemented with 10%FCS.

Construction of recombinant transfer vectors and isolation of recombinant baculoviruses expressing mutant VP7 proteins. Mutations in VP7 were made in the baculovirus transfer vector pAcCL29 (37), using synthetic oligonucleotides and the methoddescribed by Kunkel et al. (35). The wild-type BTV-10 VP7 wasderived from the transfer vector pAcYM1.10BTV7 (48). The oligonucleotidesused for mutagenesis and the resulting amino acid changes areshown in Table 1. All the oligonucleotides represent the coding-strandcomplement, with mutated anticodons underlined. The arginine residue(Arg-168) in the BTV-10 VP7 gene was mutated to alanine to createpAcCL29BTV10.7R168A. A second mutation was also introduced toconvert the aspartic residue (Asp-170) to glutamine or leucinein pAcCL29BTV10.7RD170AQ and pAcCL29BTV10.7RD170AL, respectively.The alterations in the recombinant plasmids were verified by sequenceanalyses (59). The Lipofection technique was used to cotransfectmonolayers of Sf9 cells with recombinant transfer vectors andBsu36I triple-cut A. californica nuclear polyhedrosis virus DNA(34). Recombinant baculoviruses were selected on the basis oftheir LacZ-negative phenotypes, plaque purified, and propagatedas described elsewhere (34). Three recombinant viruses, AGD,AGQ and AGL, were selected for further investigation.

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TABLE 1. Oligonucleotide primers used in site-directed mutagenesis

SDS-PAGE and Western blot analyses. The protein samples were boiled in protein dissociation buffer (10 mM Tris-HCl [pH 6.8], 10% [vol/vol] $beta$ -mercaptoethanol,10% [wt/vol] sodium dodecyl sulfate [SDS], 25% [vol/vol] glycerol,0.02% [wt/vol] bromophenol blue) at 100°C for 10 min and resolvedby SDS-polyacrylamide gel electrophoresis (PAGE) (10% polyacrylamide)followed by staining with Coomassie Brilliant blue. For Westernblot analyses proteins were transferred from gels onto a polyvinylidenedifluoride membrane by standard blotting procedures. The membraneswere incubated with an anti-BTV-10 antiserum diluted 1:1,000 inblocking buffer containing 5% (wt/vol) skimmed milk and 0.05%(vol/vol) Tween 20 in phosphate-buffered saline (PBS) and thenwith a secondary antibody conjugated with alkaline phosphataseand developed with the alkaline phosphatase substrate (NBT-BCIP[GIBCO-BRL] in 0.1 M Tris-HCl [pH 8.5]-0.1 M NaCl-0.05M MgCl₂).

Purification of recombinant VP7 protein and BTV CLPs. The wt and mutant BTV-10 VP7 proteins were purified as described previously (1). The infected Sf9 cells were infected witheither AcBTV10.7 or one of the three recombinant viruses (AGD,AGQ, and AGL) at a multiplicity of infection of 5 PFU per cell,harvested at 48 h postinfection, washed in PBS, resuspended incold TNN (100 mM NaCl, 50 mM Tris-HCl [pH 8.0], 0.5% Nonidet P-40),and homogenized at 4°C as described above. Cell debris and nucleiwere precipitated by centrifugation (10 min at 16,000 × g). Ice-coldsaturated ammonium sulfate in 100 mM Tris-HCl (pH 7.5) was addedto the cytoplasmic cell extracts to a final concentration of 20%.The protein was precipitated by centrifugation, resuspended in10 mM Tris HCl (pH 8.5), isolated from the insoluble materialfollowing removal by pelleting at 10,000 × g for 10 min, and thendialyzed against the same buffer at 4°C overnight. The extractwas stored at $-$ 20°C prior toanalysis.

Baculovirus-expressed CLPs were purified as described previously (17). In brief, Sf9 cells were coinfected with AcBTV17.3virus and the mutant VP7 baculoviruses at a multiplicity of infectionof 5 PFU per cell. After incubation at 28°C for 48 h, the cellswere harvested and the baculovirus-expressed CLPs were purifiedby a sucrose gradient (66%, [wt/vol] and 30% [wt/vol]) centrifugation.The recovered CLPs were analyzed for the presence of VP3 and VP7proteins by SDS-PAGE (10% polyacrylamide) and Western blot analysisusing anti-BTV-10 polyclonal antibodies, and the morphology wasverified byEM.

Production of MAbs against BTV VP7. Female BALB/c mice were inoculated intraperitoneally three times, at 2-week intervals, with 100 µl of either sucrose gradient-purifiedbaculovirus-expressed recombinant wt CLP or partially purifiedbaculovirus-expressed recombinant VP7 at a concentration of ~500µg/ml. The animals were rested for 3 weeks before intravenousinoculation with a further 100 µl of the same protein. Their spleenswere removed 3 days later. Fusions were carried out by using polyethyleneglycol 1500 (BCL) and the myeloma cell line SP2/o (16). VP7-specificantibody production was detected and verified by indirect ELISA,indirect immunofluorescence, and Western blotting using recombinantVP7 antigen and other baculovirus recombinant proteins as a control(18). Antibody-positive clones were isolated and maintainedin RPMI 1640 (GIBCO) with 15% Myoclone Super Plus fetal calf serum(GIBCO). Peritoneal macrophages were added to these cultures toassist growth of the clones. Mouse ascites were induced by intraperitonealinoculation of 10⁶ to 10⁷ hybridoma cells in BALB/c mice pretreated with 0.5 ml of pristane(2,6,10,14-tetramethylpentadecane) 3 to 6 days prior to theinoculation.

Antibody purification. Anti-BTV-10 VP7 antibodies in ascitic fluid (AF) were purified using an affinity chromatography kit (Pharmacia). AF was diluted1:1 with binding buffer and centrifuged at 1,000 × g for 5 minto remove large protein aggregates. After sterilization usinga 0.45-µm-pore-size Millipore filter, the AF was purified by affinitychromatography using a Pharmacia Biotech Mab Trap G II kit. Thecolumn was equilibrated with 3 ml of binding buffer (0.2 M sodiumphosphate [pH 7.0]). The sample was loaded to bind the immunoglobulinG (IgG) to the protein G in the column via the Fc region. Contaminantswere removed from the column by washing with 5 ml of binding buffer.The bound IgG was eluted with 3 ml of elution buffer (1.0 M glycine-HCl[pH 2.7]) and immediately neutralized with 75 µl of 1.0 M Tris-HCl(pH 9.0) per ml of purifiedIgG.

Production of Fab fragments. A 100-µl volume of each purified antibody was incubated at 37°C for 2 h with 100 µl of 0.02-mg/ml papain attached to beadedagarose (Sigma). The reaction was stopped by addition of 20 µlof 300 mM iodoacetamide. Complete fractionation was monitoredby SDS-PAGE (10% polyacrylamide) examination of theproduct.

ELISA. Conventional ELISA procedures were performed as described previously (9). In brief, Micro ELISA plates were coated overnightwith an optimal concentration of antigen (10 µg/well) in carbonatecoating buffer (15 mM Na₂CO₃, 36 mM NaHCO₃ [pH 9.6]) and subsequentlyblocked with PBS supplemented with 2% (wt/vol) skim milk. Incubationof primary antibody in serial two or fivefold dilutions was followedby incubation with alkaline phosphatase-conjugated secondary antibody(anti-mouse IgG [Sigma] diluted 1:500 in PBS). The reaction wasdeveloped by adding the substrate (1 mg/ml of disodium- $rho$ -nitrophenylphosphate [pNPP; Sigma] in 100 mM glycine-1 mM MgCl₂-1 mM ZnCl₂[pH 10.4]), and stopped with 3 N NaOH; the optical density wasread at 405nm.

EM and immunogold labeling. Purified wt and mutant CLPs were resuspended in water, and 10-µl drops of CLPs were absorbed onto carbon-coated copper 400mesh EM grids for 15 min, washed with water, and negatively stainedwith 2% (wt/vol) uranyl acetate. The grids were examined in aJEOL 100CX electron microscope at 100kV.

For immunogold labeling, grids with absorbed CLPs were floated first on a blocking solution of 0.1% (wt/vol) bovine serumalbumin BSA in PBS for 15 min and then processed as follows: (i)15 min on a droplet of the appropriate VP7 monoclonal antibody(AF diluted in 1:500 PBS containing 0.1% BSA), followed by threequick washes in PBS; (2) 15 min on a droplet of gold particles(diameter, 5 nm) conjugated to goat anti-mouse IgG and IgM antibody(British Biocell International) diluted 1:20 in PBS containing0.1% BSA, followed by three quick washes in PBS; and (iii) 40s in 2% uranyl acetate. The grid was then blotted and air dried.In between each stage, the grids were carefully blotted onto filterpaper by holding the grid perpendicular to the paper. In eachexperiment, negative control grids with no VP7 antibody and anonspecific antibody were also prepared. For a positive control,mouse anti-CLP polyclonal antibody was used. The grids were examinedas above, and images were obtained on Agfa Scientia Electron Microscopefilm and developed in Kodak D19 for 3.5min.

Cryo-EM. The Fab-CLP complexes were made by incubating the CLPs with Fab for 1 h at room temperature with regular vortexing. The complexeswere then incubated at 4°C overnight. For complete decorationof all VP7 epitopes, a twofold excess of Fab was added for eachVP7 molecule. Specimens were prepared for cryo-EM using standardprocedures (13). A 4-µl aliquot of the specimen was appliedto one side of a holey carbon grid. This grid was then blottedand plunged into a bath of liquid ethane ( $-$ 180°C). The frozen-hydratedsample was transferred to a precooled low-temperature cryoholderand observed in either a JEOL 1200 or Philips CM120 transmissionelectron microscope. Regions of interest were imaged at ×30,000and ×28,000 magnification, respectively with an electron doseof 5 electrons/Å². From each region, a focal pair was recorded with intended defocusvalues of 1.2 and 2.4 µm. The electron images were recorded witha 1-s exposure on Kodak SO-163 films. The films were developedin Kodak D-19 developer for 12 min at 21°C and fixed in Kodakfixer for 10min.

3D structural analysis. Micrographs were selected based on particle concentration, quality of ice, and appropriate defocus. The images were digitizedon a Zeiss SCAI microdensitometer (Carl Zeiss, Inc., Englewood,Colo.) using a 7-µm step size. The pixels were then averaged togive a 14-µm step size, which corresponded to 4.67 Å/pixel inthe object for the JEOL microscope or 5.0 Å/pixel in the objectfor the Philips microscope. CLP-antibody complexes were extractedwith a suitable box size. The determination of the orientationalparameters, their refinement, and the 3D reconstructions wereproduced by ICOS Toolkit software suite using standard procedures(11). Three-dimensional reconstruction, from a set of particles,which adequately represented the icosahedral asymmetric unit,was computed using cylindrical expansion methods. The further-from-focusmicrograph in each focal pair was processed first to obtain alow-resolution reconstruction, and this was then used to assistin finding correct orientations for the particles imaged in thecorresponding closer-to-focusmicrograph.

The reconstructions of the various particles were computed to a resolution within the first zero of the contrast transferfunction of the corresponding micrograph. The reconstructionswere viewed on a Silicon Graphics Workstation using IRIS Explorerv3.5 (Numerical Algorithms Group, Inc.).

Direct binding of CLPs onto KC cells. Confluent monolayers of KC cells (63) were prepared in 96-well culture plates. KC cells were seeded at 10⁶ cells per well and grown overnight at 28°C in Schneider mediumsupplemented with 5% FCS. Before the cells were used for bindingto CLPs, the cell medium was removed from each well. The KC cellswere washed with prechilled PBS-0.1% sodium azide to a final concentrationof 10 µg/ml. To each well, 50 µl of the diluted CLPs were addedand the absorption was allowed to continue for 30 min at roomtemperature. The cells were washed three times with prechilledPBS before being fixed with prechilled 90% ethanol-10% PBS for10 min and subsequently washed three times with prechilled PBS.To each well of fixed cells, 100 µl of blocking buffer (1% skimmilk in PBS) was added, and the cells were incubated for 1 h at37°C and washed three times with PBS before detection of CLP binding.CLPs bound to the cells were detected by two types of antibodies,the polyclonal BTV-10 antibody and MAb H1.4 diluted with PBS containing0.5% skim milk and 0.05% Tween 20 to final dilutions of 1:1,000and 1:5,000, respectively. CLP-adsorbed cells in each well wereincubated with 50 µl of the respective antibody for 1 h at 37°Cand washed three times with PBS prior to the addition 50 µl ofanti-mouse antibody-alkaline phosphatase conjugate. Antibody bindingon adsorbed CLPs was detected similarly to the detection usedin the normal ELISA procedure described above. Each experimentwas repeated at least threetimes.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Mutagenesis of the unique RGD motif of VP7 does not alter the overall antigenic and biochemical characteristics of VP7. RGD domains are involved in the binding of viruses to the cell membrane. The X-ray structural analysis of VP7 and BTV coreshas revealed that an RGD motif is accessible on the surface ofthe 38-kDa VP7 molecule (Fig. 1) and likely to be antigenic todetermine the antigenic nature and to assess the role of the RGDmotif in cell binding, mutations targeting this tripeptide weredesigned that did not perturb either the VP7 monomer-monomer orthe trimer-trimer interactions in the core assembly. In one, theRGD site was changed to AGD by changing arginine at 168 positionto alanine. In one of the two remaining double mutants, arginine168 is replaced by alanine and aspartate 170 is replaced by glutamine,converting the RGD site to AGQ, and in the other, arginine 168is replaced by alanine and aspartate is replaced by leucine generatingthe sequence AGL. The rationale for creating the mutant motifsis that the AGQ motif is found at the equivalent position in theclosely related AHSV-4 VP7 (2), suggesting that it should supportcell entry, whilse the AGL mutant has precedent. Mutant VP7 DNAswere used to generate three recombinant baculoviruses, VP7-AGD,VP7-ADQ, and VP7-AGL, each with an altered VP7 molecule. To demonstratethat the recombinant RGD-mutated VP7 proteins were expressed ininsect cells, extracts of Sf9 cells infected with the differentbaculoviruses were analyzed by SDS-PAGE. The expression of mutantVP7 molecules was examined by SDS-PAGE and compared with the baculovirus-expressedwt VP7 (48). As shown in Fig. 2A, a protein band of 38 kDa wasidentified for each of the RGD mutants (lanes 2 to 4). Both thelevels of expression and sizes of the mutant proteins were similarto those of VP7 (lane 1). The authenticity of each mutant VP7was further confirmed by Western blot analyses using an availablepolyclonal antiserum raised to BTV10-VP7. As shown in Fig. 2B,all three mutant proteins (lanes 2 to 4) reacted with the polyclonalantibody as well as with wt-VP7 (lane 1), indicating that thesemutants retained the overall molecular and antigenic propertiesof the VP7 protein.

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FIG. 1. Alpha carbon trace representation of BTV-10 VP7 with RGD site indicated. The VP7 trimer is made up of three monomers (purple, grey, and yellow), and the position of the RGD triplet within a short beta strand (cyan) is shown on the grey monomer. Detail of RGD triplet and the surrounding sequence are shown in exploded view as a ball-and-stick model.

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FIG. 2. Expression of wt and mutated VP7 proteins. Sf9 cells were infected with Ac10BTV.7, expressing the wt (lane 1) or mutated (VP7-AGD [lane 2], VP7-AGQ [lane 3], and VP7-AGL [lane 4]) VP7 proteins. (A) The infected-cell lysates were analyzed by SDS-PAGE (10% polyacrylamide) and stained with Coomassie brilliant blue. (B) The proteins were electroblotted onto a membrane and reacted with BTV-10 polyclonal antisera. The arrow indicates the size of wt and mutated VP7 proteins. The protein mass markers are indicated on the left.

One of the striking features of BTV VP7 is that it oligomerizes readily into a trimeric form both in solution and in crystals(1), which are the building blocks for core assembly (36).Since the RGD residues are located in a loop on the VP7 upperdomain, not at the interface between VP7 monomers, the mutatedVP7 proteins should not perturb the monomer-monomer interactions.To confirm that the VP7 mutants still retained the ability toform trimers, we purified each expressed VP7 mutant and investigatedtheir oligomeric nature using an assay system that we developedpreviously (36). All three mutants formed trimers which couldbe detected by SDS-PAGE (data not shown), confirming that substitutionwithin the RGD motif did not alter the interface regions of theVP7 mutants. Similarly, circular dichroism analysis of the purifiedrecombinant proteins showed no discernible change in the spectraof the RGD site-mutagenized VP7 proteins compared to spectra ofunmodified VP7, indicating that the RGD mutations had no overalleffect on the secondary elements ( $alpha$ helix or $beta$ strand) of VP7 (datanotshown).

VP7 molecules with mutations at the RGD site interact with VP3 and assemble into CLPs that are morphologically indistinguishable from normal CLPs. Since the RGD site is located on the upper domain of the protein and is not in contact with the underlying scaffolding VP3layer, the mutated VP7 molecules should still assemble into CLPsin the presence of the VP3 molecule. Therefore, to determine this,we used a coexpression system in which assembly of CLPs was assessedby coinfection of insect cells with the recombinant virus expressingeither wt VP7 or one of the three VP7 mutants and a recombinantvirus expressing authentic VP3 molecules. The assembled CLPs werepurified through a sucrose gradient and analyzed by SDS-PAGE.As shown in Fig. 3A, two protein bands at 120 and 38 kDa, representingVP3 and wt (lane1) or RGD-mutated (lanes 2 to 4) VP7s, respectively,were observed for each CLP preparation. Both protein bands reactedspecifically in the immunoblot with polyclonal antiserum raisedto BTV-10 virus (Fig. 3B). This indicates that the mutated VP7proteins were still able to assemble into CLPs when coexpressedwith VP3. The morphology of the CLP prepared by each mutant VP7was further analyzed by EM, which revealed that the RGD-mutatedCLPs formed from VP7-AGD, VP7-AGQ, and VP7-AGL exhibited the samesize and morphological features as did the wt CLPs formed withunmodified VP7 (Fig. 3C). The RGD-mutated CLPs appeared highlystable upon storage at 4°C in 0.2 M Tris (pH 8.0) for prolongedperiods (more than 2 months).

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FIG. 3. CLP formation by VP3 and wt or mutated VP7 proteins. Sf9 cells were coinfected with baculoviruses expressing VP3 with either the wt VP7 or various VP7 mutants. The CLPs were purified as described in Materials and Methods. (A and B) The CLPs were analyzed by SDS-PAGE (10% polyacrylaride) and stained with Coomassie brilliant blue (A) or immunoblotted with polyclonal Ab to BTV-10 (B). The arrows indicate the sizes of VP3 and mutated VP7 proteins. (C) CLP formation was confirmed by electron microscopy. Bars, 100 nm.

These data indicate that the mutations at Arg-168 and Asp-170 do not interfere with the interaction with VP3 and could formstable CLPs that are structurally similar to the nativeCLPs.

Identification of MAbs targeted to the RGD site of VP7 molecule. To determine further the accessibility of the RGD motif in the BTV core and to map the antigenic region of VP7, a panel of12 VP7 MAbs (MAbs H1.2 to H1.11 and CLPIII) that reacted specificallywith native VP7 antigen as well as with CLPs were generated asdescribed in Materials and Methods. Further, to determine whetherthese MAbs are targeted to the upper domain of VP7, their reactivitieswith two previously generated domain-switched VP7 chimeric constructs(45) were assessed by ELISA and Western blot analysis. One ofthese consists of only the upper domain of BTV VP7, while thelower domain is derived from the AHSV (ABA) VP7 molecule, andthe second is a reverse construct (BAB) in which the upper domainis replaced by the fragment of AHSV VP7 but the lower is BTV VP7.The antibodies showed no cross-reactivity with either the purifiedAHSV VP7 protein or the purified BAB VP7 but reacted with ABAVP7 protein as strongly as with the wt BTV VP7 (Fig. 4A), demonstratingthat all MAbs are targeted to the upper domain of VP7 molecule.

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FIG. 4. ELISA of the wt, chimeric, and mutant VP7 proteins. Micro-ELISA plates were coated with the purified recombinant proteins. A panel of six VP7 MAbs (H1.2 to H1.6 AND CLPIII) was tested with all the antigens, using 1:1,000 to 1:24,000 dilutions of sera. The optical density (OD) reading at 405 nm of a 1:10,000 dilution of each MAb is shown. (A) The micro-ELISA plates were coated with either the wt (

) or one of the two domain-switched chimeric, ABA (

), BAB (

) VP7. (B) Micro-ELISA plates were coated with either the wt (

) or the RGD mutants, AGD (

), AGL (

), AGQ (

To identify whether any of these MAbs specifically mapped to the RGD site of the VP7 molecule, each MAb was subsequently assessedfor its binding ability to each of the purified RGD substitutionmutants is an ELISA. As shown in Fig. 4B, 3 of the 12 MAbs (H1.5,H1.6, and CLPIII) did not bind to the RGD mutated VP7 proteins,although all the other MAbs bound to some degree; this suggeststhat at least three MAbs are specifically targeted to the regionof the RGD site. This is probably because this site is particularlyimmunogenic.

To evaluate the accessibility of the RGD motif in the BTV core and to confirm further that H1.5 and CLPIII indeed recognizethe RGD site of the molecule, CLPs generated with each of theRGD mutants as well as with native VP7 molecule were examinedfor their binding ability to these MAbs by immuno-EM. As shownin Fig. 5, immunogold staining of the mutants with these two MAbsproduced similar results. There was no binding of antibodies ofH1.5 or CLPIII to the CLPs generated with the VP7-AGQ mutant (Fig.5A). However, immunogold-labeled MAb H1.4 bound successfully toADQ-CLP (Fig. 5B). This indicates that MAbs H1.5 and CLPIII, butnot H1.4, are targeted to the RGD site in VP7. Similar resultswere obtained with the other two VP7-AGD and VP7-ADL mutants (datanot shown). Further, ELISA using CLPs assembled with each VP7mutant molecule confirmed that H1.5 and CLPIII do not bind tothe CLPs that were generated with the three mutants but boundto the wt CLPs strongly (data not shown).

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FIG. 5. Immunogold labeling of CLPs with VP7 MAb H1.5. CLPs formed with VP3 and wt VP7 or VP7-AGQ were immunogold labeled with MAb, followed by the secondary antibody (goat anti-mouse) coupled with 10-nm-diameter gold particles. The complexes were visualized by EM. Bars, 100 nm. (A) wt CLPs showing the gold particles bound to the surface of CLPs; (B) CLPs formed by the VP7-AGQ, with no gold particles bound.

Visualization of CLP-antibody complexes by high-resolution cryo-EM. The immunogold labeling studies showed that CLPIII and H1.5 had reduced binding to the CLPs containing VP7 with mutated RGDsequence compared with binding to the wt CLPs. This suggested,therefore, that these antibodies bound to a site which includedthe RGD epitope of VP7. Several methods can provide informationconcerning the region of antibody binding to the particles, includingcryo-EM and 3D image reconstruction, which allow visualizationof the antigen-antibody complexes at relatively high resolution(26). Therefore, to gain some insight into the antibody bindinglocation on CLPs, we have generated CLP-H1.5/CLPIII Fab complexesas described in Materials and Methods and have examined theseby cryo-EM and 3D image reconstruction. Sufficient Fabs were addedto the CLPs that optimal antibody decoration of the VP7 moleculescould be achieved without a large excess of Fab, which could interferewith the reconstruction. The decorated particles were well separatedin ice and were homogeneous in appearance, as shown in Fig. 6A.As expected, the decorated particles had a different appearancefrom undecorated CLP. A halo of even thickness surrounding eachparticle (Fig. 6A) was observed that completely obscured the VP7trimers. The VP3 subcore layer could be seen as a dark ring inthe particle images. The decorated particles were ~140 Å largerin diameter than the undecorated particles, resulting in a totaldiameter of ~840 Å. These particles were used for 3D image reconstruction.The radial-density plot (data not shown) was calculated from the3D reconstruction to represent the protein components at variousradii within the 3D structure. By comparing this radial-densityplot with that of the WT CLP reconstruction, it was evident thatattached to the VP7 layer of the CLP was a layer of extra densitywhich extended to a radius of ~420 Å. This density has been attributedto the bound antibody molecules. It is clear in Fig. 6B that theextra density, attributed to Fab (yellow), sits on the surfaceof the CLP. An equatorial slice of the reconstruction revealsthat the Fab is attached to the upper domain of the VP7 (blue)(Fig. 6C). Density due to the Fab was seen extending from alltrimers in the particle. The removal of radial sections correspondingto Fab density revealed the VP7 directly beneath the antibodylayer. This layer of protein was largely unchanged in conformationor position (Fig. 6B).

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FIG. 6. Cryon-EM of the CLP-H1.5 complex. (A) Micrograph of the CLP-H1.5 complex. An arrow indicates the diffuse electron density surrounding the particle. The arrowhead indicates a ring due to the smooth inner shell formed by the VP3 layer. The inset shows the CLPs without the MAb. (B) Surface representation of CLP-H1.5 complex viewed down the threefold axis. The decorated particle has a radius of ~420 Å. The antibody fragments are shown in yellow. The VP7 trimers to which the antibodies attach are colored blue. The VP3 layer is exposed to the surface of the particle at the fivefold axes and is colored green. (C) Equatorial slice of the reconstruction (~47 Å thick). Note that the antibody fragments (yellow) are bound to the upper domain of the VP7 (blue).

RGD mutations inhibit CLP binding to KC cells, and MAbs targeted to RGD compete with CLP binding. To assess whether the RGD site plays a role in core entry, we have developed an assay system to investigate the cell bindingability of CLPs as representatives of BTV cores. In this assay,Culicoides-derived KC cells, which are permissive for BTV coreinfection, are used as an immobilized layer and the binding ofboth wt and mutant CLPs is assessed following incubation by anELISA using either polyclonal BTV antibody (Fig. 7A) or MAb H1.4,a MAb (Fig. 7B) whose binding is not affected by the RGD mutations.Using this assay format, wt CLPs were found to bind to KC cellsin a dose-dependent manner (Fig. 7) irrespective of the serumused for detection. In contrast to wt CLPs however, CLPs generatedwith the VP7-RGD mutants showed only a low-level binding to thecell surface and failed to show a significant dose-response curve.These data are consistent with a role for the RGD sequence ofVP7 in cell binding.

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FIG. 7. Binding of wt and RGD-mutated CLPs to KC cells in binding ELISA. KC cells were grown in 96-well plates, and wt and RGD-mutated CLPs were allowed to bind. The CLP attachment was detected as described in Materials and Methods. The amount of CLP bound is expressed as the optical density (OD) at 405 nm and is plotted against increasing CLP concentrations (0 to 250 µg), and the bound CLP was detected by polyclonal BTV-10 antibody (A) or MAb H1.4 (B). Note the high level of binding for the wt CLP ( $black-lozenge$ ) with the increasing concentration of CLPs but no increase of binding with the same concentrations of CLPs for VP7-AGD ( $black-triangle$ ), VP7-AGQ (

), and VP7-AGL ( $open circle$ ). The data plotted represent the average of three experiments performed in parallel. The standard deviation at a given point was no more than 7% of the value shown.

To confirm a role for the VP7 RGD motif, a second series of cell binding assays were carried out. In these, the binding activityof CLPs to KC cells was determined in the presence of MAb H1.5,a MAb whose epitope includes the RGD site of VP7. Following incubationof a fixed concentration of CLPs with different amounts of H1.5,residual CLP binding to the cell surface was detected by ELISAusing a BTV polyclonal antibody. The addition of MAb H1.5 competedwith the cell binding ability of CLPs, which increased significantlyas the concentration of MAb decreased (Fig. 8). The addition ofMAb to RGD mutant CLPs had no effect on the low level of cellbinding observed. The data obtained with MAb H1.5 competitionare consistent with a role for the RGD motif of VP7 in CLP bindingto the KC cell surface and, by implication, with the entry ofBTV cores into Culicoides cells.

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FIG. 8. Binding of wt and RGD-mutated CLPs to KC cells in the presence of MAb H1.5. KC cells were grown in 96-well plates, 100 µg of either wt or RGD-mutated CLPs was bound in the presence of increasing dilutions of MAb H1.5 (1:500 to 1:10,000), and the bound CLPs were detected using polyclonal BTV-10 antibody as described in Materials and Methods. The experiment were carried out three times for each preparation. The average amount of CLP bound in three experiments is expressed as the optical density (OD) at 405 nm and is plotted against decreasing MAb dilutions. The bound CLPs are indicated as follows: $black-lozenge$ , wt;

, KC cells; $black-triangle$ , VP7-AGD;

, VP7-AGQ; $open circle$ , VP7-AGL.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

BTV-VP3 and VP7 proteins self-assemble into empty CLP when coexpressed in insect cells by using recombinant baculoviruses(17). Assembled CLPs mimic the authentic virus cores and providean in vitro model for direct structure-functional studies. Inthis study we examined the effect of point mutations introducedinto VP7 on virus-host protein interactions. The expression ofrecombinant capsid proteins and their assembly into virus-likeparticles have been similarly used to study virus-host interactionin binding and internalization of bovine papillomavirus (46),Norwalk virus (64), and rotaviruses (15).

Comparative sequence data and structural studies have implicated the RGD tripeptide sequence in BTV-VP7 (amino acid residues168 to 170) in virus attachment to Culicoides host cells. To date,however, little direct evidence has been available to test thishypothesis for BTV even though RGD is critical for other virus-receptorinteractions. To provide direct evidence for VP7 RGD tripeptideinvolvement in virus attachment, we introduced point mutationsat amino acid residues 168 and 170, converting RGD to either AGD,AGQ, or AGL. The coexpression of RGD-mutated proteins with BTV-VP3in the baculovirus system resulted in the assembly of CLPs andshowed no gross change in the overall conformation by the introductionof mutations in this region. The assembled CLPs formed by theseRGD-mutated VP7s appeared equivalent to authentic BTV cores inmorphological, biochemical, and overall immunological characteristics.This view is supported by three sets of experimental data: (i)RGD-mutated VP7 proteins reacted with anti-BTV serum in immunoblotassays as did the wt; (2) RGD-mutated VP7 proteins were structurallysimilar to wt VP7, as indicated by the similarity in secondarystructures from CD analysis and their ability to oligomerizationinto trimers, a feature of the VP7 molecule; and (iii) the assembledCLPs were structurally and functionally equivalent to the authenticCLPs. Since no gross change of structure occurred by mutationof RGD, the role of the sequence in host cell binding was assessed.A direct approach, in which CLPs were assayed by indirect ELISAfor binding to the surface of Culicoides (KC) cells, indicatedthat alteration of the RGD sequence led to a reduced level ofCLP binding. An indirect approach, in which MAbs raised againstVP7 were used as competitor for CLP binding, showed that onlyMAbs that mapped directly to the RGD motif gave effective competition.MAbs that bound the upper domain of VP7 but were not affectedby mutations at RGD did not compete for KC cell surface binding.Together, these data indicate that the RGD motif of BTV VP7 isaccessible in the context of the CLP (MAb generation and cryo-EMdecoration) and is responsible for cell surface binding. The RGDtripeptide is conserved for all BTV serotypes of VP7s as wellas for EHDV, despite the location of the motif in an exposed position,where antibody-selected variation might be expected to occur (31,54, 68). The RGD motif of AHSV is located in a slightly differentposition from that of BTV but also on a highly flexible and exposedloop (2). Moreover, the structure of the integrin insertionregion, domain I, can be easily docked onto the RGD motif of bothBTV and AHSV VP7 proteins (3).

There is accumulating evidence for the involvement of an RGD or an RGD-like tripeptide amino acid sequence in virus bindingto cellular integrins during infection by a number of viruses.The role played by these tripeptide-containing ligands could beindirect, as is the case for adenovirus (4, 12, 47, 65),or direct, as for rotaviruses (10, 21, 27), papillomoviruses(14), and members of the Picornaviridae family, including echoviruses1, 8, and 9 (5, 30, 49, 60, 70); coxsackievirus A9(7, 8, 53, 61); FMDV (6, 32, 50, 51); and humanparechovirus (62). It has been shown conclusively that the RGDmotif in FMDV is essential for virus entry, since mutations inthis sequence, including the conservative change to RGE, resultedin noninfectious virus particles that failed to enter cells (39-41).Recent extensive analysis of the mechanism of rotavirus cell entryhas shown that such tripeptides do indeed act as ligands for integrinsand that peptides containing these sequences and MAbs againstintegrins block the entry and infectivity of rotavirus (21,27, 69). Using CLPs as a model system for cell binding, VP7mutants were assessed for their cell attachment capability andthe data obtained demonstrated clearly that mutated CLPs eitherdid not bind to Culicoides-derived cells at all or bound at muchreduced level compared to the wt CLPs, suggesting a role for RGDin core uptake by the insectcells.

MAbs specific for integrins that recognize the RGD sequences of viral proteins block virus attachment and infectivity of otherviruses (33, 52, 61, 62). In our study we have used theVP7 MAbs that are RGD site specific (e.g., H1.5 and CLPIII) toblock the CLP attachment and have demonstrated that such MAbsinterfere with CLP binding to KC cells. Cryo-EM analysis has shownthat Fab fragments of these MAbs decorate the surface of the CLPseffectively and that FAbs bind to a region which includes theRGD site. Together, the data support the hypothesis that the VP7RGD motif, as presented in associated with VP3, is at least partof the receptor binding sequence of BTVcores.

	ACKNOWLEDGMENTS

We thank T. Booth, IVEM, Oxford, United Kingdom, and D. Stuart, Oxford University, Oxford, United Kingdom, for their supportand advice on structural work, and we are grateful to B. V. V.Prasad, Baylor College, Houston, Tex., for providing the cryo-EMfacility. We also thank M. Gross, New Chemistry Laboratory, Universityof Oxford, for assistance in circular dichroismanalysis.

This work was partly funded by grants from the BBSRC (United Kingdom) and NIH (UnitedStates).

	FOOTNOTES

^* Corresponding author. Present address: Department of Infectious and Tropical Diseases, London School of Hygiene and TropicalMedicine, Keppel St., London WC1E 7HT, United Kingdom. Phone:44 20 7927 6239. Fax: 44 20 7636 8739. E-mail: polly.roy{at}lshtm.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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69. Zárate, S., R. Espinosa, P. Romero, C. A. Guerrero, F. Arias, and S. López. 2000. Integrin $alpha$ 2 $beta$ 1 mediates the cell attachment of the rotavirus neuraminidase-resistant variant nar3. Virology 287:50-54.

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