Substitutions at the Putative Receptor-Binding Site of an Encephalitic Flavivirus Alter Virulence and Host Cell Tropism and Reveal a Role for Glycosaminoglycans in Entry

doi:10.1128/JVI.74.19.8867-8875.2000

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Journal of Virology, October 2000, p. 8867-8875, Vol. 74, No. 19
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Substitutions at the Putative Receptor-Binding Site of an Encephalitic Flavivirus Alter Virulence and Host Cell Tropism and Reveal a Role for Glycosaminoglycans in Entry

Eva Lee and Mario Lobigs^*

Division of Immunology and Cell Biology, John Curtin School of Medical Research, Australian National University, Australian Capital Territory, Australia

Received 3 May 2000/Accepted 10 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The flavivirus receptor-binding domain has been putatively assigned to a hydrophilic region (FG loop) in the envelope (E)protein. In some flaviviruses this domain harbors the integrin-bindingmotif Arg-Gly-Asp (RGD). One of us has shown earlier that hostcell adaptation of Murray Valley encephalitis virus (MVE) canresult in the selection of attenuated variants altered at E proteinresidue Asp₃₉₀, which is part of an RGD motif. Here, a full-length,infectious cDNA clone of MVE was constructed and employed to systematicallyinvestigate the impact of single amino acid changes at Asp₃₉₀on cell tropism, virus entry, and virulence. Each of 10 differentE protein 390 mutants was viable. Three mutants (Gly₃₉₀, Ala₃₉₀,and His₃₉₀) showed pronounced differences from an infectious clone-derivedcontrol virus in growth in mammalian and mosquito cells. The alteredcell tropism correlated with (i) a difference in entry kinetics,(ii) an increased dependence on glycosaminoglycans (determinedby inhibition of virus infectivity by heparin) for attachmentof the three mutants to different mammalian cells, and (iii) theloss of virulence in mice. These results confirm a functionalrole of the FG loop in the flavivirus E protein in virus entryand suggest that encephalitic flaviviruses can enter cells viaattachment to glycosaminoglycans. However, it appears that additionalcell surface molecules are also used as receptors by natural isolatesof MVE and that the increased dependence on glycosaminoglycansfor entry results in the loss ofneuroinvasiveness.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Virus attachment to the host cell is the first stage of the virus replication cycle. It requires the molecular interactionbetween the virion surface and a host cell receptor and is oftenthe basis for viral species and tissue tropisms as well as virulenceproperties. The cellular receptors for some viruses have beendefined and reveal diverse strategies for virus attachment, rangingfrom binding to specific cell surface proteins to attachment viawidely distributed carbohydrate moieties, such as sialic acidand heparan sulfate (for a review, see reference 48). For alarge number of viruses, however, specific host cell receptorshave not been identified. The use of multiple receptors on individualor different cells could be one reason for this lack of knowledge.This scenario has been proposed for the attachment of flaviviruses(35), a genus of approximately 70 mainly arthropod-borne, envelopedRNA viruses. Most flaviviruses replicate in vertebrate and arthropodcells and exhibit a wide species and tissue tropism. Numerouscandidate receptor proteins with a molecular mass of 40 to 80kDa have been found to associate with flaviviruses in bindingassays (19, 22, 27, 36, 44). Furthermore, an importantrole of heparan sulfate has also been demonstrated for the attachmentof dengue-2 virus to vertebrate cells (7). Interestingly, cellsurface glycosaminoglycans (GAGs) are exploited as attachmentmolecules by other viruses in a process thought to concentratevirus particles at the cell surface for subsequent binding tohigh-affinity receptors (for a review, see reference 2). Noexperimental evidence on the use or nature of a high-affinityreceptor for any of the flaviviruses exists atpresent.

Flavivirus attachment and entry are mediated by the envelope (E) protein (~50 kDa), the major glycoprotein on the flavivirusparticle (for reviews, see references 6 and 33). The E proteinforms an oligomer with the small membrane (M) protein (~8 kDa)and constitutes most of the accessible virion surface; this isreflected in the dominance of the E protein as target antigenfor virus-neutralizing and protective antibodies (33). The definitionof the crystal structure of the ectodomain of the E protein ofthe flavivirus tick-borne encephalitis virus (TBE) (37), incombination with phenotypic analyses of E protein variants, hasshed light on functional domains and mechanisms involved in flavivirusattachment and entry (for a review, see reference 33). An investigationby one of us on genotypic changes associated with host cell adaptationof the encephalitic flavivirus Murray Valley encephalitis virus(MVE) suggested an important role for residue 390 in the E proteinin cell tropism and virulence (25). Asp₃₉₀ found in the prototypevirus was altered to His, Gly, Ala, or Asn after passage of MVEin a human adenocarcinoma (SW13) cell line, resulting in improvedgrowth in the human cell line as well as virulence attenuationin mice. Residue 390 in the E protein of MVE is part of an Arg-Gly-Asp(RGD) sequence, the integrin-binding motif important in cell-extracellularmatrix and cell-cell adhesion (42). This evidence prompted thefirst proposition for the location of the flavivirus receptor-bindingsite in a conserved, hydrophilic domain encompassing residue 390,with a possible role for integrins in the attachment of some flaviviruses(25). However, the RGD motif is not found in the E protein ofall flaviviruses: it is found in Japanese encephalitis virus (JEV)(31), yellow fever virus (YFV) strain 17D (39), and the relatedRGE/T sequences in other members of the JEV serocomplex (5,8, 47), but the corresponding amino acids in the E proteinof the dengue viruses are unrelated (12, 26, 30) and deletedin TBE (29). Intriguingly, the RGD sequence in the vaccine (17D)strain of YFV (39) arose as a consequence of host cell adaptationof the virulent Asibi strain, which has the corresponding aminoacids Thr-Gly-Asp (11). Based on these sequence comparisons,it is unlikely that integrins are a general receptor for flavivirusattachment, in contrast to foot-and-mouth disease virus (16,34) and coxsackievirus (40), which display a strict dependenceon RGD-mediated integrin binding for host cellentry.

The crystal structure of the TBE E protein strongly supports a function in receptor binding of the hydrophilic region whichharbors the RGD motif of some flaviviruses. This sequence is foundin a solvent-exposed (FG) loop located in the immunoglobulin-likedomain III of the E protein, and mutations which affect host celltropism and virulence in different flaviviruses map in this region(37). In the current study, we introduced substitutions at theRGD motif in MVE with the use of an infectious clone. The phenotypiceffects of changes in the putative flavivirus receptor-bindingdomain on virus growth, attachment, and entry in cultured cellsand virulence in mice wereexamined.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses and cells. The MVE prototype strain MVE-1-51 (9) has been passaged 15 times in suckling mouse brain; a culture supernatant from C6/36cells was used as workingstock.

Vero (African Green monkey kidney), BHK-21 (baby hamster kidney), and SW13 (human adenocarcinoma) cells were all from theAmerican Type Culture Collection (Bethesda, Md.) and maintainedin Eagle's minimal essential medium (EMEM) plus nonessential aminoacids and 5% fetal calf serum (FCS). C6/36 (Aedes albopictus)cells were grown in EMEM plus nonessential amino acids and 7%FCS at 28°C.

Plasmids. DNA fragments comprising the 5' or 3' half of the genome of MVE-1-51 were obtained by reverse transcription (RT)-PCR usingexpand reverse transcriptase and the Expand high-fidelity PCRsystem (both from Roche Diagnostics, Castle Hill, NSW, Australia).Oligonucleotide primers used in RT-PCR were designed to incorporatethe promoter sequence for T7 RNA polymerase plus an ApaI restrictionendonuclease recognition site (underlined) at the 5' terminus(5'-GCTTGGGCCCTAATACGACTCACTATAAGACGTTCATCTGCGTGAGCTTCCGATCTCAG-3')and a NotI site (underlined) at the 3' terminus (5'-TATGCGGCCGCAGATCCTGTGGTCTTCTCCCCCAT-3')(nucleotides in italics are not present in the viral genome).Two additional internal primers corresponded to sequences encompassinga unique BamHI site (underlined) in the middle of the genome (sense,5'-GGAACTTCAGGATCCCCAATAGTCAATAGC-3'; antisense, 5'-GCTATTGACTATTGGGGATCCTGAAGTTCC-3').RT-PCR fragments 5,057 and 6,024 bp in size and correspondingto the 5' and 3' portions of the genome, respectively, were produced.Plasmids pM110, pM210, and pM310 were generated by ligation ofindependently produced 5' 5,057-bp fragments, after digestionwith ApaI and BamHI, into plasmid pBR322* (2,793 bp) digestedwith the same enzymes and treated with shrimp alkaline phosphatase(Roche Diagnostics). This vector was derived from pBR322 by deletionof a 1,666-bp fragment encoding tetracycline resistance betweenthe EcoRI and BspEI sites and insertion of the polylinker frompBluescript KS+ (Stratagene, La Jolla, Calif.) at the site ofdeletion. Plasmids pM116, pM211, pM212, pM213, and pM215 containthe full-length MVE cDNA. They were generated by ligation of independentlyproduced 3' 6,024-bp fragments cut with BamHI and NotI into pM110or pM210 digested with the same enzymes. Plasmids pM312' and pM312"were produced by replacement of the MVE 5' terminus of clone pM212with a 1,971-bp ApaI-XbaI fragment from pM310 or the adjacentsequence of 3,073 bp with an XbaI-BamHI fragment from pM310,respectively.

Introduction of mutations at codon 390 in the E protein gene. A shuttle vector, pM212(X/B), was made by cloning a 3,073-bp XbaI-BamHI fragment from pM212 into pBluescript II KS+ and subsequentdeletion of the polylinker region between ApaI and BamHI by digestionwith the two restriction endonucleases, treatment with T4 DNApolymerase to create blunt ends, and religation. To produce aGly₃₉₀ mutant, a 563-bp PstI-SacI fragment from pM212(X/B) wasexchanged with that obtained from RT-PCR amplification of nucleotides1,593 to 5030 in the genome of MVE-1-51 passage variant P4/10(25). The mutation was subcloned into pM212 by exchange of a3,073-bp XbaI-BamHI fragment with that containing the mutatedE protein 390codon.

A random site-directed mutagenesis approach for generating E protein 390 variants was employed with the use of the degeneratemutagenesis oligonucleotide 5'-GATTGATCTGCTTC/ANNTCCGCGGCCTACCACAAT-3',which is complementary to a sequence in the MVE E gene from nucleotides2121 to 2154 and contains the sequence for a SacII site (underlined).A 563-bp PstI-SacI fragment (nucleotides 1950 to 2513 in the MVEgenome) from pM212 was cloned into M13mp19 phage replicative form(RF) DNA for preparation of uridinylated single-stranded DNA fromrecombinant phage particles after infection of Escherichia colistrain CJ236. Mutagenesis was done as described (45); briefly,uridinylated single-stranded DNA (0.5 µg) was annealed with phosphorylatedoligonucleotide (1 pmol) and converted into RF DNA using Sequenase(5 U; USB Corp., Cleveland, Ohio) and T4 DNA ligase (2 U; PharmaciaBiotech, Uppsala, Sweden). Plaques obtained following transfectionof E. coli strain TG1 with the mutagenesis mix were screened byrestriction enzyme digestion of RF DNA and tested for the presenceof a SacII site. The DNA was then subjected to sequence analysisusing the Big-Dye terminator cycle-sequencing kit (PE AppliedBiosystems, Foster City, Calif.) to detect mutations at codon390. Mutations which gave rise to amino acid changes were clonedas PstI-SacI fragments from RF DNA samples into the transfer vectorpM212(X/B) digested with the same enzymes prior to transfer intofull-length clone pM212 as describedabove.

Transcription of RNA from full-length MVE cDNA clones. Plasmids containing the full-length MVE cDNA were digested with NotI and treated with Klenow fragment (Pharmacia Biotech)to create blunt ends. After extraction with phenol-chloroformand ethanol precipitation, linearized DNA was added to a transcriptionmix containing 0.5 U of T7 RNA polymerase (Promega, Madison, Wis.)and 1 U of RNase inhibitor (RNAGuard; Pharmacia Biotech, Uppsala,Sweden) per µl, 40 mM Tris-HCl (pH 7.9), 6 mM MgCl₂, 2 mM spermidine,10 mM NaCl, 10 mM dithiothreitol, 1 mg of bovine serum albumin(BSA) per ml, 1 mM CAP analogue mG(5')ppp(5')G (Pharmacia Biotech),and 1 mM each ATP, UTP, and CTP. The mixture was incubated at37°C for 5 min, GTP was added to 1 mM, and the incubation wascontinued at 37°C for 1 h. RNA transcripts were used directlyin transfectionexperiments.

Transfection of BHK-21 and C6/36 cells. Transfection of BHK-21 cells was done by electroporation. Subconfluent cell monolayers were harvested with trypsin, washedtwice in serum-free EMEM, and suspended in EMEM at 1.2 × 10⁷ cells/ml. The cells (10⁷) were mixed with in vitro-synthesized RNA in an electroporationchamber (0.4-cm gap; Life Technologies, Rockville, Md.) and subjectedto two consecutive pulses at 250 V, 800 µF, and "low-ohm" settingusing the Cell-Porator electroporation system I (Life Technologies).Cells were left at room temperature for 5 min, suspended in 24ml of EMEM-5% FCS, and transferred to culture dishes for incubationat 37°C. Culture fluids were harvested after 3 days for plaqueisolation and titration. For RNA transfection of C6/36 cells,lipofectin (6 µl; Life Technologies) was mixed with 0.4 ml ofphosphate-buffered saline (PBS) and held at room temperature for15 min, and then RNA transcript (0.2 µg) was added, and the mixturewas applied to cells in a 35-mm dish (washed twice with PBS).After incubation at room temperature for 20 min, the transfectionmix was removed, monolayers were washed once with PBS, and EMEM-7%FCS wasadded.

Virulence assays. Virulence assays were performed in 3-week-old Swiss White outbred mice as described (32). Virus stocks used in virulenceassays were obtained by plaque purification on Vero cells followedby two rounds of amplification in C6/36 cells. Virus samples wereserially diluted in Hanks' balanced salt solution (HBSS) containing20 mM HEPES (pH 8.0) plus 0.2% BSA (HBSS-BSA), and 30 µl was inoculatedinto each animal by the intracranial (i.c.) or intraperitoneal(i.p.)route.

Infectivity assays. Vero cells (2 × 10⁵/well) and SW13 cells (10⁵/well) in 24-well Linbro dishes (ICN Biomedicals, Aurora, Ohio) were infected at~0.1 PFU/cell, the virus was left to adsorb for 1 h at 37°C, andmonolayers were washed twice with PBS before EMEM-5% FCS (1 ml)was added. At 16, 20, 24, and 28 postinfection (hpi), the culturesupernatant was collected and stored at $-$ 70°C following the additionof HEPES buffer (pH 8.0) to 10 mM. Monolayers were washed oncewith PBS, and fresh medium (1 ml) was added. Virus growth samplesfrom Vero and SW13 cells were titrated by plaque formation onVero or SW13 cell monolayers, respectively, using six-well Linbrotrays (ICN Biomedicals). Overlay medium for plaque assay containedEMEM plus 1% agar (Difco Laboratories, Irvine, Calif.) and 2%FCS in both cases. Plaques on Vero cells were visualized by addingneutral red stain (ICN Biomedicals; 0.02% [wt/vol] in 1% agarsolution) at 4 to 5 days postinfection (dpi). Plaques on SW13cells were visualized at 5 dpi after removal of agar overlay andstaining with crystal violet (0.1% in 20% ethanol-H₂O).

For virus growth assays in C6/36 cells, monolayers (2 × 10⁵ cells/well) in 24-well trays were infected with 0.1 C6/36 focus-formingunit/ml. After 1 h of adsorption, the monolayers were washed and1 ml of EMEM-7% FCS was added. The cells were incubated at 28°C.Virus growth samples were collected between 20 and 42 hpi as above.Virus titration was performed by an immunofluorescence focus assayon C6/36 cell monolayers in 24-well dishes. Overlay medium containedEMEM-5% FCS-1% carboxymethyl cellulose (high viscosity; ICN Biomedicals;prepared as a 3% stock solution in water and autoclaved). At 3dpi, monolayers were washed with PBS and fixed in ice-cold acetone-methanol(1:1). Foci of infection were detected using an anti-MVE hyperimmuneascitic fluid, fluorescein isothiocyanate-conjugated anti-mouseimmunoglobulin G (IgG), (Silenus Laboratories, Hawthorn, Australia)and immunofluorescencemicroscopy.

Virus attachment and entry assays. For uptake assays, SW13 cell monolayers (60% confluent) in six-well trays were used after replacing the medium with HBSS-BSA.Virus samples (200 SW13 PFU in HBSS-BSA) were added to each wellat room temperature. At specified times after virus addition,monolayers were washed three times with acid EMEM (pH 4.0, bufferedwith 20 mM [2-N-morpholino]ethane-sulfonic acid; ICN Biomedicals).The monolayers were incubated with acid medium for 2 min, andthe medium was aspirated and replaced with HBSS-BSA. The acidtreatment inactivates bound and unbound virus but not virus whichhas undergone uptake by endocytosis (10, 18). Overlay agarwas then added, and cells were incubated for 5 days to allow plaquedevelopment. A control monolayer for each virus sample was usedfor plaque titration in the absence of the acidtreatment.

To confirm that bound but noneclipsed virus was completely inactivated by the acid treatment, SW13 cell monolayers (60% confluent)in six-well Libro trays were cooled to 4°C for 30 min after replacingmedium with HBSS-BSA. Virus samples (400 SW13 PFU in HBSS-BSA)were added to each well, and incubation was continued at 4°C for60 min. Unbound virus was removed by two washes of the monolayerswith HBSS-BSA, and acid treatment was performed as above. Themonolayers were left under HBSS-BSA for a further 10 min at 37°Cprior to the addition of an agar overlay (see above) and incubatedfor 5 days at 37°C to allow plaque development. For each virussample, a control monolayer which was not subjected to acid treatmentwasincluded.

Heparin inhibition of virus attachment. The effect of heparin on MVE infection of Vero, SW13, and BHK-21 cells was assayed by preincubation of virus samples (100to 200 PFU in 100 µl of HBSS-BSA) with heparin (20 to 200 µg/ml;Sigma, St. Louis, Mo.) for 15 min prior to addition to cell monolayers(incubated with 200 µl of HBSS-BSA containing 20 to 200 µg ofheparin per ml). After 1 h, agar overlay medium (see above) wasadded to allow plaquedevelopment.

The effect of heparin on virus attachment was assayed in Vero and SW13 cells by preincubation of virus samples (400 PFU in100 µl of HBSS-BSA) at 4°C with heparin (20 to 200 µg/ml) priorto addition to chilled (4°C, 30 min) cell monolayers (incubatedwith 200 µl of HBSS-BSA containing 20 to 200 µg of heparin perml) followed by incubation on ice for 1 h. Unbound virus was removedby two washes of the cell monolayers with HBSS-BSA, and the monolayerswere held at 37°C for 10 min before addition of an agaroverlay.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Full-length infectious cDNA clones of MVE-1-51. cDNA fragments corresponding to the 5' and 3' halves of the MVE genome and overlapping at a unique BamHI site at nucleotide5010 were generated by RT-PCR. A 5' ApaI restriction site, a T7RNA promoter sequence, and a 3' NotI site were incorporated intothe PCR primers to allow cloning of PCR fragments into a low-copy-numberplasmid (pBR322*) and in vitro synthesis of full-length RNA transcript.These transcripts contain an authentic 5' end but six additionalnucleotides (NotI site) at the 3' end (Fig. 1). Five full-lengthMVE cDNA clones (pM116, pM211, pM212, pM213, and pM215) comprisingtwo of the three independently derived 5' halves and five independentlyderived 3' halves of the genome were generated. Two additionalclones were produced from the third 5' half of the MVE genomeby replacement of the MVE 5' end of clone pM212 with a 1,971-bpApaI-XbaI fragment (pM312') or the adjacent sequence of 3,073bp with an XbaI-BamHI fragment (pM312"). All plasmids encodingthe full-length MVE cDNA were stably propagated in E. coli MC1061.1cells but required incubation for 30 h at 37°C for sufficientyield.

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FIG. 1. Full-length infectious cDNA clone of MVE-1-51. Plasmid pM212 contains the full-length cDNA of MVE-1-51 (11,013 nucleotides), which includes an open reading frame (ORF) encoding a polyprotein of 3,434 amino acids (solid line). Restriction sites used in subcloning and genetic manipulations are shown (numbering is from the 5'-terminal nucleotide in MVE-1-51). Sequences at the 5' (plus an ApaI site and T7 promoter sequence) and 3' (plus a NotI site) termini of the viral genome are shown (boxed). The vector pBR322* is a deleted version of pBR322 (see Materials and Methods). The ampicillin resistance gene (Ap), the ROP gene, and the origin of DNA replication (ORI) are shown. NCR, noncoding region.

In vitro-synthesized RNA transcripts were first tested for infectivity in mosquito (C6/36) cells using a Lipofectin-basedtransfection protocol (~0.5 µg RNA/10⁶ cells). RNA transcripts from four clones (pM212, pM213, pM215,and pM312') gave rise to progeny virus and MVE-specific immunofluorescencefoci in the monolayers at 3 days posttransfection (Table 1).RNA transcript derived from five of the seven full-length cDNAclones were also tested for infectivity in vertebrate (BHK-21)cells transfected by electroporation (~1 µg of RNA/10⁷ cells). Progeny virus was recovered for transcripts from threeclones (pM116, pM212, and pM213; Table 1). Infectivity of thedifferent RNA transcripts in C6/36 cells did not fully correspondto that in BHK-21 cells (e.g., clones pM116 and pM312'). Thiswas not investigated further but was probably due to the low infectivityof the transcripts, resulting in variable success in the productivetransfection of cells. Plasmid pM212, which gave rise to the highestinfectious titers in both BHK-21 and C6/36 cells in the initialscreening procedure, was selected for use in the subsequent experiments.The transfection efficiency of RNA derived from this clone was~100 infectious centers/µg of RNA in both cell lines tested. Thisvalue was more than 1,000-fold lower than that observed in similartransfections of C6/36 and BHK-21 cells using MVE virion RNA (~2× 10⁵ infectious centers/µg of RNA); it was also significantly lowerthan the infectivity of RNA derived from YFV (38) or TBE (28)cDNA clones but comparable to or greater than the transfectionefficiencies of RNA transcripts from other flavivirus cDNA clones(17, 20, 23, 46). Since virus progeny produced in cellstransfected with MVE cDNA clone pM212-derived RNA had growth andvirulence properties similar to those of the parent virus (seebelow), it appears that replication results in the repair of adefect present in the in vitro-synthesized genomic RNA. This couldinvolve removal of some of the additional nucleotides at the 3'end of infectious clone-derived RNA.

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TABLE 1. Infectivity of MVE full-length cDNA clone-derived RNAs in mammalian and insect cells

MVE mutants with substitutions at residue 390 in the E protein. Asp₃₉₀ in the MVE E protein is part of an RGD motif in the putative flavivirus receptor-binding domain. It is subject to replacementwith other amino acids as a result of host cell adaptation ofMVE and is also a determinant for virulence in mice (25). Toinvestigate the impact of single amino acid changes at this siteon cell tropism, virus entry, and virulence in the context ofan otherwise identical genetic background, the codon for Asp₃₉₀in MVE full-length clone pM212 was mutated to that for one of10 other amino acids. A random mutagenesis approach was used whichrelied on a degenerate oligonucleotide to introduce randomizedcodons at residue 390 as well as silent substitutions generatinga unique SacII site. A Gly₃₉₀ mutant was produced by substitutinga cDNA fragment encompassing codon 390 in pM212 with that obtainedby RT-PCR amplification from a variant virus (P4/10) which hadbeen selected by passage in SW13 cells (25). The collectionof E protein 390 mutants obtained is shown in Table 2. It includesthe conservative replacement of Asp₃₉₀ with Glu and the nonconservativesubstitutions with small aliphatic residues (Gly or Ala), aliphatichydrophobic residues (Val or Leu), an aliphatic polar residue(Thr), an aromatic polar residue (Tyr), an acidic amide (Gln),a polar weakly basic residue (His), and a basic residue (Lys).A clone unchanged at Asp₃₉₀ but with silent mutations introducingthe SacII site was also generated.

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TABLE 2. Mutations at codon 390 in the E protein and biological properties of mutants

RNA was transcribed from each of the 11 mutated full-length clones and transfected into BHK-21 cells. Culture fluids werecollected after 3 days and tested for the presence of infectiousvirus by plaque titration on Vero cells. Each of the E protein390 mutants gave rise to viable progeny virus; however, theirplaque morphology differed markedly (Table 2). In particular,the His₃₉₀ and Gly₃₉₀ viruses produced very small plaques. Mutantvirus stocks were obtained after amplification of single plaquesonce each in C6/36 and Vero cells, with the exception of the His₃₉₀and Gly₃₉₀ viruses, which were amplified twice in C6/36 cellsto obtain stocks of sufficiently high titers. The sequences fromnucleotides 960 to 2500 encompassing the entire E protein genewere confirmed for each of the mutants by direct sequencing onRT-PCR fragments obtained from intracellular RNA extracted fromcells used for virusamplification.

Growth of E protein 390 mutants in vertebrate and invertebrate cells. A previous investigation demonstrated that the substitution of Asp₃₉₀ with His in the E protein of MVE resulted in alteredvirus growth in Vero and SW13 cells (25). Although the nucleotidesequences of the E protein genes of the passage variant and prototypevirus were otherwise identical, the presence of differences elsewherein the genome could not be excluded. To confirm that residue 390is part of an E protein domain that functions as a determinantof host cell tropism and to extend this study to a wide rangeof amino acid substitutions at residue 390, ten 390 mutants withotherwise identical genetic backgrounds were examined for growthin Vero, SW13, and C6/36 cells. Infections were performed at 0.1PFU/cell in one-step growth experiments. Virus titers of growthsamples were determined on the corresponding cell lines by plaque(Vero and SW13) or immunofluorescence focus assays and (C6/36).

Growth in Vero cells of infectious clone (pM212)-derived virus vM212 and the control Asp₃₉₀ mutant virus was compared withthat of prototype virus MVE-1-51. At each time point between 16and 28 hpi, similar extracellular virus titers were detected inthe single-step growth curves for these viruses (Fig. 2).

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FIG. 2. Growth of E protein 390 mutants in cell culture. Vero, SW13, and C6/36 cells were infected with MVE-1-51, the Asp₃₉₀ control virus, or 1 of 10 E protein 390 mutants at multiplicity of ~0.1, determined for each cell type. Unbound virus was removed after 1 h of adsorption, and growth medium was added. At 16, 20, 24, and 28 hpi, supernatants were collected from Vero and SW13 cells for titration of virus infectivity, in the respective cell types. For growth assays in C6/36 cells, supernatant samples were taken at 24, 28, and 44 hpi, and virus titers were determined as focus-forming units (FFU) by immunofluorescence in C6/36 cells. Results for Vero and SW13 growth assays are from two separate experiments (shown in different graphs).

Growth of the E protein 390 mutants was tested in two separate experiments in both Vero and SW13 cells with repeat determinationsof growth phenotypes of Gly₃₉₀ and His₃₉₀ viruses shown for comparison(Fig. 2). In Vero cells all E protein 390 mutants showed lowertiters between 16 and 28 hpi than the Asp₃₉₀ virus. Two of themutants (Gly₃₉₀ and His₃₉₀) produced titers more than 100-foldbelow those of the Asp₃₉₀ virus. The other six mutants had intermediategrowth properties, with titers often reduced 10-fold. The conservativeAsp₃₉₀-to-Glu mutation gave growth properties most similar tothose of the Asp₃₉₀ virus, reaching identical titers at 28 hpi.There was a strict correlation between plaque size of the mutantson Vero cell monolayers and growth phenotypes (Table 2). In thetwo growth assays shown, the monolayers were fixed at 24 hpi fordetection of the number of virus-infected cells by immunofluorescenceassay. There was little or no difference in the percentage ofMVE-infected cells between any of the mutants tested (data notshown).

Most of the changes at residue 390 in the E protein resulted in (up to 100-fold) improved growth in SW13 cells compared tothe Asp₃₉₀ virus (Fig. 2). Highest titers were observed for theGly₃₉₀ and His₃₉₀ mutants, the two viruses that grew most poorlyin Vero cells. There was little or no difference in the numberof infected cells between all viruses tested, as determined byimmunofluorescence staining for MVE antigen at 24 hpi (data notshown).

The single-step growth curves of infectious clone-derived viruses vM212 and Asp₃₉₀ in C6/36 cells were indistinguishable fromthat of prototype virus MVE-1-51 (data not shown). Subsequently,the growth properties of five E protein 390 mutants were comparedto that of the Asp₃₉₀ virus in the mosquito cell line (Fig. 2).There was no detectable virus release at 20 hpi. At later timepoints, titer of two mutants, Gly₃₉₀ and His₃₉₀, were 20- to 100-foldlower than those for the Asp₃₉₀ control virus. The Gln₃₉₀ virusshowed intermediate growth, and titers for the Val₃₉₀ and Thr₃₉₀mutants were only slightly lower than titers for the Asp₃₉₀ control.Accordingly, the effect of different amino acid changes at residue390 in the E protein on virus growth in Vero and C6/36 cells showeda similarpattern.

Effect of residue 390 in the E protein on entry kinetics into SW13 cells. The entry kinetics into SW13 cells of the His₃₉₀ mutant, which showed improved growth in this cell line, was compared to thatof the Asp₃₉₀ control virus. Following incubation of virus oncell monolayers at room temperature for 5, 15, 30, and 60 min,unbound virus was removed and bound but noneclipsed virus wasinactivated by the addition of acidic (pH 4.0) medium. Agar overlaymedium was added, and plaques were allowed to develop over 5 days.The acid wash induces an irreversible conformational change inthe E protein (1) which inactivates virus infectivity (10,18). This was corroborated in control experiments, in whichplaque formation was completely inhibited when adsorption wasperformed at 4°C for 1 h prior to the addition of acid medium.The kinetics of virus entry of the His₃₉₀ mutant was significantlyfaster than that of the Asp₃₉₀ virus, with greater than twofolddifferences seen at all time points (Fig. 3). Similar resultswere obtained in two repeat experiments. These data suggest thatamino acid substitutions at residue 390 can result in more efficientvirus uptake into SW13 cells. Consequences of enhanced uptakekinetics would be (i) a faster growth kinetics and (ii) an increasein the relative infectivity in the cell line used to generatethe single-step growth curves. Collectively, these factors arelikely to account for the improved growth phenotypes of most Eprotein 390 mutants observed in SW13 cells.

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FIG. 3. Uptake of MVE into SW13 cells. The kinetics of uptake of the Asp₃₉₀ control and His₃₉₀ mutant viruses into SW13 cells was determined as described in Materials and Methods. Percent uptake for each time point is expressed as the ratio of the number of plaques obtained after acid treatment and the number of plaques obtained on a control monolayer in the absence of acid treatment.

Differential inhibition of virus infectivity by heparin is determined by amino acids at residue 390 in the E protein. The improved entry kinetics into SW13 cells of one of the E protein 390 mutants relative to the control virus, the selectionof amino acid changes at residue 390 during host cell adaptationof MVE (25), and the location of residue 390 in a domain withputative receptor-binding function (25, 37) suggest a criticalrole for this site in virus attachment to host cell receptors.Given that host cell adaptation of some other viruses correlatedwith an increased dependence on GAGs in virus attachment (3,21, 43) and that a role for GAGs in dengue-2 virus attachmentto vertebrate cells has been documented (7), we tested theeffect of heparin on infection of Vero, SW13, and BHK cells withprototype MVE and E protein 390 mutantviruses.

Heparin had little effect on the infectivity of MVE-1-51 in Vero and SW13 cells. Preincubation of a virus inoculum (~200 PFU)with heparin at high concentrations (200 to 400 µg/ml) reducedplaque numbers by <20% in Vero and ~25% in SW13 cells (data notshown). The control Asp₃₉₀ virus and the Gly₃₉₀, His₃₉₀, and Lys₃₉₀mutants were similarly tested using heparin concentrations from50 to 200 µg/ml (Fig. 4A). The Asp₃₉₀ virus showed <5% reductionin plaque numbers in Vero cells at all heparin concentrationstested, up to 28% reduction in plaque numbers in SW13 cells, and30 to 60% plaque reduction in BHK-21 cells. In contrast, the Gly₃₉₀mutant showed a much greater sensitivity to heparin inhibition.Plaque numbers in Vero cells were reduced by up to 80%, in SW13cells by 70 to 88%, and in BHK-21 cells by 50 to 80% dependingon the dose of heparin used. The His₃₉₀ mutant showed 5 to 20%reduction in plaque numbers in Vero cells at 50 to 200 µg of heparinper ml and a greater reduction in SW13 cells (60 to 80%) and BHK-21cells (28 to 95%). The infectivity of the Lys₃₉₀ mutant was asor less susceptible to inhibition by heparin as the Asp₃₉₀ controlvirus (5% in Vero, 5 to 20% in SW13, and 10 to 40% in BHK-21 cells).

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FIG. 4. Inhibition by heparin of virus infectivity in Vero, SW13, and BHK cells. (A) The Asp₃₉₀ control and His₃₉₀, Gly₃₉₀, and Lys₃₉₀ mutant viruses (200 PFU) were incubated with heparin (0, 50, 100, and 200 µg/ml) prior to their addition to cells pretreated with HBSS-BSA containing heparin at 0, 50, 100, or 200 µg/ml. Agar overlay was added to allow plaque formation after 1 h of adsorption at 37°C. Inhibition by heparin was calculated using the formula [(plaque number on nontreated cells $-$ plaque number on heparin-treated cells)/(plaque number from non-treated cells)] × 100. (B) Inhibition of infectivity by heparin (200 µg/ml) of 10 E protein 390 mutants was assayed in parallel with the Asp₃₉₀ control virus as in panel A. The percent inhibition by heparin of the Asp₃₉₀ virus is subtracted from that for the E protein 390 mutants obtained in the same experiment. Results (mean and standard error) from three independent experiments are shown for each mutant. (C) Inhibition by heparin of virus binding to Vero and SW13 cells. The Asp₃₉₀ control virus and the His₃₉₀ mutant were incubated with heparin (0, 20, 50, 100, or 200 µg/ml) for 15 min at 4°C and then added to chilled Vero or SW13 cells treated with heparin (0 to 200 µg/ml). After 1 h of adsorption at 4°C, cell monolayers were washed, and agar overlay was added to allow plaque development. Percent inhibition by heparin is calculated as in panel A. Results (mean and standard error) from two independent experiments are shown.

The effect of heparin on infectivity was then tested for each of the 10 E protein 390 mutants in comparison to the controlAsp₃₉₀ virus using 200 µg of heparin per ml (Fig. 4B). Positivevalues indicate reduction in plaque numbers above and negativevalues indicate reduction below that with the Asp₃₉₀ control virus.In addition to the Gly₃₉₀ and His₃₉₀ mutants, infectivity of theAla₃₉₀ mutant in Vero and SW13 cells was also inhibited significantlymore by heparin than that of the Asp₃₉₀ virus (Fig. 4B). The othermutants tested were not significantly different from the Asp₃₉₀virus (Glu₃₉₀ and Gln₃₉₀) or were somewhat less sensitive to heparininhibition in SW13 cells (Thr₃₉₀, Lys₃₉₀, and Tyr₃₉₀). The susceptibilityto heparin inhibition of SW13 cell infectivity of the Val₃₉₀ andLeu₃₉₀ viruses was marginally greater (~20%) than that of theAsp₃₉₀ virus (reproduced in threeexperiments).

Heparin inhibits entry of MVE into Vero and SW13 cells. To confirm that heparin inhibits virus binding or entry into cells, an entry assay was performed (Fig. 4C). Ice-cold mixturesof virus (Asp₃₉₀ control or His₃₉₀ mutant virus) and heparin (20to 200 µg/ml) were added to chilled Vero or SW13 cell monolayersand held for 1 h at 4°C for binding to occur without uptake byendocytosis. We found that the effect of heparin on virus infectivitywas markedly increased when virus adsorption was performed at4°C and the heparin-treated virus inoculum was completely removedprior to the addition of an agar overlay (compare Fig. 4A andC). The infectivity of the His₃₉₀ mutant was inhibited by morethan 50% at 20 and 200 µg of heparin per ml in SW13 and Vero cells,respectively. In contrast, the inhibition by heparin of entryof the Asp₃₉₀ control virus resulted in a plateau of not greaterthan 50% reduction of infectivity in both cell lines, suggestingthat the Asp₃₉₀ virus can enter these cell lines by a mechanismwhich does not involve virus binding to cell surface GAGs. Itis notable that Vero cells were significantly less susceptiblethan SW13 cells to inhibition by heparin in both binding and infectivityassays (Fig. 4A and C), suggesting a greater dependence on GAGsof MVE entry into SW13 than Verocells.

Virulence of E protein 390 mutants. Mouse virulence of full-length MVE clone (pM212)-derived virus vM212 was determined by inoculating 3-week-old Swiss outbredmice with 10-fold serial dilutions of plaque-purified virus stocki.c. or i.p. (24, 32). Comparison of i.c. versus i.p. 50%lethal dose (LD₅₀) values, which did not differ by more than 10-fold,showed that vM212 was virulent (Fig. 5). The Asp₃₉₀ virus whichwas used as a control for the other infectious clone-derived variantswas also virulent by this criterion. Of the six E protein 390mutants tested for mouse virulence, the Glu₃₉₀, Gln₃₉₀, and Thr₃₉₀mutants were also considered virulent. The Gly₃₉₀ and His₃₉₀ mutantswere attenuated, as they induced no mortality by i.p. inoculationdespite having i.c. LD₅₀ values (<50 PFU) similar to that of theAsp₃₉₀ virus. The Tyr₃₉₀ mutant showed an approximately 100-folddifference between the i.c. and i.p. LD₅₀ values and is consideredintermediate in virulence.

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FIG. 5. Virulence of infectious clone-derived MVE and E protein 390 mutants. Virus stocks were diluted 10-fold serially in HBSS-BSA and used to inoculate 21-day-old Swiss outbred mice in groups of five by the i.p. or i.c. route. Mortality was recorded for 14 days.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Functional role of the putative flavivirus receptor-binding domain in cell tropism and attachment/entry. We have examined the functional role of the putative flavivirus receptor-binding domain in virus entry, host cell tropism,and pathogenesis in mice. In the E protein of MVE, this domaincontains the RGD integrin-binding motif. The codon for Asp₃₉₀,which is part of the RGD motif, was targeted by site-directedmutagenesis using a full-length cDNA clone. Infectious clone-derivedcontrol virus vM212 was indistinguishable from the prototype virus,MVE-1-51, in growth in Vero cells and virulence in mice. All Eprotein 390 mutants were viable and produced plaques in Vero,SW13, and BHK-21 cells; however, marked differences in growthproperties were observed. Replacement of Asp₃₉₀ with small aliphatic(Gly or Ala) or a weakly basic (His) amino acid resulted in themost significant changes in virus growth; a 50- to 100-fold reductionin growth in Vero and C6/36 cells and >10-fold enhancement ofgrowth in SW13 cells was seen in comparison with an Asp₃₉₀ controlvirus. The other mutants showed smaller differences, but growthin Vero cells was always less efficient than that of the Asp₃₉₀virus and comparable or improved in SW13 cells (Table 2). Theobservation that MVE is largely tolerant to a wide range of changesat the third amino acid of the RGD motif suggests that these changesdo not alter the structure of the E protein such that replicationin cultured cells is inherently impaired. This contrasts withthe neighboring Gly₃₈₉, which, when replaced with Ala, destabilizesthe structure of the E protein in YFV 17D (49). A Gly is foundat the corresponding position in almost all flaviviruses, whereasAsp₃₉₀ (MVE E protein sequence numbering) is not highly conserved.A comparison of the efficiencies of RNA synthesis of wild-typeand E protein 390 variants has revealed no significant differencewhen identical numbers of cells were infected (A. Thompson andL. Dalgarno, personalcommunication).

Analysis of E protein 390 mutants confirmed the significance of this residue as a determinant of host cell tropism. Giventhat residue 390 is located in the putative receptor-binding domain(7, 37), the most likely functional consequence of substitutionsat this position is an altered receptor interaction. Interestingly,the most pronounced changes in growth phenotypes were found forthree mutants which were described in an earlier study of MVEvariants selected by serial passage in SW13 cells (25). However,most SW13-passaged variants had other changes in the E proteinin addition to the substitution of Asp₃₉₀. In the present investigationthe derivation of the Gly₃₉₀, His₃₉₀, and Ala₃₉₀ mutants froman infectious clone ascertained an otherwise identical geneticbackground.

In this study we provide conclusive evidence that the putative flavivirus receptor-binding domain is a functional determinantfor virus entry into cells. Previous work has given suggestivesupport for the involvement of this domain in attachment and entry.First, variants of MVE with altered host cell tropism and virulenceproperties had substitutions at residue 390 (25), located ina hydrophilic region corresponding to the FG loop in the E proteincrystal structure of TBE (37). Second, neutralization escapemutants of TBE had amino acid replacements at residues 384 and387, both spatially proximal to the FG loop, and were attenuatedfor virulence in mice (13, 14). Third, based on the structureof the TBE E protein, the FG loop is exposed on the virion surfaceand meets the physical requirements for receptor binding (37).Fourth, the E proteins of several flaviviruses (e.g., MVE, JEV,and YFV) contain within the FG loop an RGD integrin-binding motif,utilized by other viruses for attachment to host cells. Mutationsleading to the loss or gain of this RGD motif were found followinghost cell adaptation by serial passaging of MVE (25) and YFV(11). Here we show that single amino acid changes in the FGloop of the E protein of MVE give rise to variants with alteredattachment and entry phenotypes in comparison with the prototypevirus. Two assays were used to analyze the early events of virusinfection. An uptake assay, in which noneclipsed virus particleswere inactivated by acid treatment, clearly demonstrated the fasterentry kinetics of a His₃₉₀ mutant relative to the control virus.The converse has been reported for Vero cells, in which the penetrationof His₃₉₀ and Ala₃₉₀ variants was found to be significantly delayedrelative to that of the parent virus, MVE-1-51 (23a). Given thatthe rate of virus uptake is most likely a consequence of the efficiencyof interaction between the virus and a host cell receptor(s),the differential entry kinetics of the two viruses suggests thatthe E protein domain encompassing residue 390 functions in virusattachment. This is strongly supported by the result of the secondattachment-entry assay, which showed a striking correlation betweengrowth properties in cultured cells and susceptibility to heparininhibition of virus infectivity, both of which were influencedby the amino acid at residue 390 in the E protein (Table 2).This is consistent with the interpretation that substitutionsat residue 390 in the putative receptor-binding domain can alterreceptor usage, as reflected in the differential involvement ofcell surface GAGs in virusentry.

Role of GAGs in entry of an encephalitic flavivirus. Heparan sulfate on the cell surface plays a role in the attachment of a number of viruses (3, 21, 41, 43), includingthat of dengue-2 virus, to mammalian cells (7, 15). GAG-mediatedvirus attachment is inhibited by heparin, a highly sulfated formof heparan sulfate. We tested whether infectivity of MVE in Vero,SW13, and BHK-21 cells was sensitive to inhibition by heparinand found a dose- and cell type-dependent effect for the prototypevirus. This inhibitory effect of heparin on virus infectivitywas significantly greater for three of the 390 mutants (Gly₃₉₀,His₃₉₀, and Ala₃₉₀). Two mutants (Val₃₉₀ and Leu₃₉₀) showed anintermediate phenotype of susceptibility to heparin, whereas theothers did not differ markedly from the Asp₃₉₀ virus (Table 2).The observation that substitutions at residue 390 in the E proteincan render MVE infectivity highly susceptible to heparin inhibitionstrongly suggests that this site is in close proximity to a GAG-bindingdomain in the E protein and can directly influence the interactionbetween virus and cell surface GAGs. Support for this interpretationhas been obtained in an investigation of JEV variants adaptedto growth in SW13 cells which had single amino acid change locatedin a loop directly opposing residue 390 according to the crystalstructure of the TBE E protein (unpublished data). Nevertheless,it cannot be excluded that substitutions at residue 390 in theMVE and JEV E proteins alter the overall conformation of the proteinand influence a distantly located domain important for virus attachmentand entry. The reason why small uncharged (Gly and Ala) or smallpolar (His) amino acids at residue 390 would enhance virus bindingto GAGs is not immediately apparent. GAG-binding domains are characteristicallyrich in basic amino acids which are flanked by hydrophobic residues(41). An attractive hypothesis is that the positively chargedArg in the RGD motif or other basic residues in a region spatiallyproximal in the protein structure bind to negatively charged GAGsand that this interaction is subject to steric and charge hindrancedepending on the amino acid at residue390.

The altered attachment and entry properties of some of the MVE E protein 390 mutants have revealed a GAG-dependent entry mechanismthat could be inhibited almost completely by heparin. However,the significance of cell surface GAGs for the entry of naturalisolates of MVE, which are unaltered in the RGD motif (24),is unclear in view of the partial inhibition of infectivity byheparin found for the prototype virus. The latter observationis consistent with the view that one or more alternative cellsurface molecules lacking heparan sulfate moieties can functionas receptors for virus attachment. We have speculated that integrinsare a candidate receptor for MVE and other flaviviruses that possessan RGD integrin-binding motif (25), but have been unable todemonstrate this interaction using RGD motif-containing peptidesin attempts to inhibit the infectivity of MVE (E. Lee, unpublisheddata). A similar conclusion was reached by van der Most et al.(49), who tested a putative function of integrins as receptorsfor YFV 17D. From the present study, it is apparent that experimentsattempting to block one specific virus-host cell receptor interactionmust take into consideration the use of alternative (e.g., GAGdependent) mechanisms for attachment and entry which may gainin significance when the first pathway isblocked.

Effect of GAG dependence in virus entry on virulence. Residue 390 in the E protein of MVE is also a determinant of pathogenesis in mice. Of six mutants tested, two (Gly₃₉₀ andHis₃₉₀) had lost neuroinvasiveness and were considered fully attenuatedby the criteria of the virulence assay. However, their growthin the brain following i.c. inoculation was not notably changed,based on the average time to death of the infected animals. Theloss of neuroinvasiveness of the Gly₃₉₀ and His₃₉₀ mutants mostlikely reflects their inefficient replication in extraneural tissues.Thus, the correlation of altered cell tropisms and of increasedsusceptibility of virus entry to inhibition by heparin with thetype of amino acid at residue 390 extends to virulence phenotypesin mice. A parallel may be drawn between the attenuated 390 mutantsof MVE and Sindbis virus variants, which were derived from cellculture adaptation, attenuated, and dependent on GAG-mediatedattachment for infectivity in cultured cells (3, 4, 21).It was argued that the loss of virulence of the Sindbis virusvariants was a consequence of their high affinity for GAGs andthat after peripheral inoculation these attenuated variants areconcentrated and inactivated in the liver, an organ highly enrichedin GAGs, thus limiting their ability to spread to the brain. Asimilar scenario has been proposed for the attenuation of foot-and-mouthdisease virus (43) and may explain the loss of neuroinvasivenessof E protein 390 mutants of MVE and other flavivirus variantsattenuated by host celladaptation.

	ACKNOWLEDGMENTS

We are grateful to L. Dalgarno and R. C. Weir for the provision of unpublished sequence data for MVE-1-51.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Immunology and Cell Biology, John Curtin School of Medical Research, AustralianNational University, P.O. Box 334, Canberra, ACT 2601, Australia.Phone: 61-2-62494048. Fax: 61-2-62492595. E-mail: Mario.Lobigs{at}anu.edu.au.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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38. Rice, C. M., A. Grakoui, R. Galler, and T. J. Chambers. 1989. Transcription of infectious yellow fever RNA from full-length cDNA templates produced by in vitro ligation. New Biol. 1:285-296[Medline].

39. Rice, C. M., E. M. Lenches, S. R. Eddy, S. J. Shin, R. L. Sheets, and J. H. Strauss. 1985. Nucleotide sequence of yellow fever virus: implications for flavivirus gene expression and evolution. Science 229:726-733[Abstract/Free Full Text].

40. Roivainen, M., L. Piirainen, T. Hovi, I. Virtanen, T. Riikonen, J. Heino, and T. Hyypia. 1994. Entry of coxsackievirus A9 into host cells: specific interactions with alpha v beta 3 integrin, the vitronectin receptor. Virology 203:357-365[CrossRef][Medline].

41. Rostand, K. S., and J. D. Esko. 1997. Microbial adherence to and invasion through proteoglycans. Infect. Immun. 65:1-8[Medline].

42. Ruoslahti, E., and M. D. Pierschbacher. 1987. New perspectives in cell adhesion: RGD and integrins. Science 238:491-497[Abstract/Free Full Text].

43. Sa-Carvalho, D., E. Rieder, B. Baxt, R. Rodarte, A. Tanuri, and P. W. Mason. 1997. Tissue culture adaptation of foot-and-mouth disease virus selects viruses that bind to heparin and are attenuated in cattle. J. Virol. 71:5115-5123[Abstract].

44. Salas-Benito, J. S., and R. M. del Angel. 1997. Identification of two surface proteins from C6/36 cells that bind dengue type 4 virus. J. Virol. 71:7246-7252[Abstract].

45. Stocks, C. E., and M. Lobigs. 1998. Signal peptidase cleavage at the flavivirus C-prM junction: dependence on the viral NS2B-3 protease for efficient processing requires determinants in C, the signal peptide, and prM. J. Virol. 72:2141-2149[Abstract/Free Full Text].

46. Sumiyoshi, H., C. H. Hoke, and D. W. Trent. 1992. Infectious Japanese encephalitis virus RNA can be synthesized from in vitro-ligated cDNA templates. J. Virol. 66:5425-5431[Abstract/Free Full Text].

47. Trent, D. W., R. M. Kinney, B. J. Johnson, A. V. Vorndam, J. A. Grant, V. Deubel, C. M. Rice, and C. Hahn. 1987. Partial nucleotide sequence of St. Louis encephalitis virus RNA: structural proteins, NS1, ns2a, and ns2b. Virology 156:293-304[CrossRef][Medline].

48. Tyler, K. L., and B. N. Fields. 1996. Pathogenesis of viral infection, p. 173-218. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed. Lippincott-Raven, Philadelphia, Pa.

49. van der Most, R. G., J. Corver, and J. H. Strauss. 1999. Mutagenesis of the RGD motif in the yellow fever virus 17D envelope protein. Virology 265:83-95[CrossRef][Medline].

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46.	Sumiyoshi, H., C. H. Hoke, and D. W. Trent. 1992. Infectious Japanese encephalitis virus RNA can be synthesized from in vitro-ligated cDNA templates. J. Virol. 66:5425-5431[Abstract/Free Full Text].
47.	Trent, D. W., R. M. Kinney, B. J. Johnson, A. V. Vorndam, J. A. Grant, V. Deubel, C. M. Rice, and C. Hahn. 1987. Partial nucleotide sequence of St. Louis encephalitis virus RNA: structural proteins, NS1, ns2a, and ns2b. Virology 156:293-304[CrossRef][Medline].
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