Replicase Complex Genes of Semliki Forest Virus Confer Lethal Neurovirulence

doi:10.1128/JVI.74.10.4579-4589.2000

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Journal of Virology, May 2000, p. 4579-4589, Vol. 74, No. 10
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Replicase Complex Genes of Semliki Forest Virus Confer Lethal Neurovirulence

Minna T. Tuittila,¹^,²^,^* Maria G. Santagati,³ Matias Röyttä,⁴ Jorma A. Määttä,¹^,² and Ari E. Hinkkanen¹^,²

Department of Biochemistry and Pharmacy, Åbo Akademi University,¹ Turku Immunology Centre,² and Department of Virology, MediCity Research Laboratory,³ and Department of Pathology,⁴ University of Turku, Turku, Finland

Received 21 April 1999/Accepted 10 February 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Semliki Forest virus (SFV) is a mosquito-transmitted pathogen of small rodents, and infection of adult mice with SFV4, a neurovirulentstrain of SFV, leads to lethal encephalitis in a few days, whereasmice infected with the avirulent A7(74) strain remain asymptomatic.In adult neurons, A7(74) is unable to form virions and hence doesnot reach a critical threshold of neuronal damage. To elucidatethe molecular mechanisms of neurovirulence, we have cloned andsequenced the entire 11,758-nucleotide genome of A7(74) and comparedit to the highly neurovirulent SFV4 virus. We found several sequencedifferences and sought to localize determinants conferring theneuropathogenicity by using a panel of chimeras between SFV4 anda cloned recombinant, rA774. We first localized virulence determinantsin the nonstructural region by showing that rA774 structural genescombined with the SFV4 nonstructural genome produced a highlyvirulent virus, while a reciprocal recombinant was asymptomatic.In addition to several amino acid mutations in the nonstructuralregion, the nsp3 gene of rA774 displayed an opal termination codonand an in-frame 21-nucleotide deletion close to the nsp4 junction.Replacement in rA774 of the entire nsp3 gene with that of SFV4reconstituted the virulent phenotype, whereas an arginine at theopal position significantly increased virulence, leading to clinicalsymptoms in mice. Completion of the nsp3 deletion in rA774 didnot increase virulence. We conclude that the opal codon and aminoacid mutations other than the deleted residues are mainly responsiblefor the attenuation of A7(74) and that the attenuating determinantsreside entirely in the nonstructuralregion.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Semliki Forest virus (SFV) is an enveloped positive-stranded RNA virus of the family Togaviridae. The SFV prototype was isolatedin 1942 from a pool of mosquitoes in Uganda (40). The A7(74)strain (4) is a derivative of an SFV strain isolated from mosquitoesin Mozambique in 1959 (26). Several strains of SFV, such asL10 (4) and SFV4 (24), cause lethal encephalitis in miceof all ages, leading to death of the animals in a few days (3,11), whereas A7(74) infection of adult mice is asymptomaticper se but leads to axonal demyelination mediated by CD8⁺ T cells (2). However, the severity of A7(74) infection isstrictly age dependent, being lethal for neonatal mice less than2 weeks old (8, 27), probably because the strain is capableof virion formation in propagating neurons, unlike in mature neurons(27).

SFV nonstructural proteins (nsP) are translated as a polyprotein (nsP1234) from the genomic 42S RNA, and they form essentialcomponents of viral RNA replication and transcription complexes(14). The nsP1 protein is a methyl- and guanylyltransferase(1, 18), whereas the nsP2 is a proteinase (45) and nucleosidetriphosphatase (33). The nsp3 gene product is a phosphoprotein,and it has been proposed to function together with nsP1 in anchoringthe replication complex proteins to cytoplasmic membrane structures(30, 31). In Sindbis virus (SIN), p123 and p1234 are producedfirst and then cleaved proteolytically. p123 and nsP4 functionin minus-strand RNA synthesis, but cleaved products from p123are required for efficient plus-strand RNA synthesis (38). Mutationsin the SIN nsP3 protein have been shown to result in blockageof RNA synthesis, indicating the importance of this protein orthe polyprotein component in replication, although the exact mechanismof action remains unknown (21). The nsp4 gene displays highsimilarity to the RNA-dependent polymerase sequences of otherRNA viruses (13, 15). Recently, enzymatically active RNA replicationmachinery was reconstructed for SIN in vitro by introducing togetherthe single components of the multiprotein complex (22).

In several alphaviruses, such as SIN, Middelburg virus (43), and Ross River virus (42), as well as Venezuelan (16) andwestern and eastern (48) equine encephalitis viruses, an opal(UGA) termination codon interrupts the polygenic RNA at the 3'end of the nsp3 gene. In contrast, in the SFV prototype (44)and in SFV4, an arginine codon is found at the analogous position.For the related O'Nyong-nyong virus, strains with either an arginine(42) or an opal codon (19) have been characterized. In RNAviruses generally, readthrough of an in-frame termination codonis often employed to regulate the synthesis of a viral polymeraseor reverse transcriptase (23). In SIN, the opal readthroughproceeds with about 20% efficiency in vitro, leading to lowernsP4 amounts (25), but rather than total nsP4, the relativeamounts of nsP3, nsP34, and nsP4 seem to be important for efficientalphavirus replication (23).

Although in many alphaviruses mutations in the virion proteins or nucleocapsid have been found to alter virulence (11, 36),often having a synergistic effect (32), the results presentedin this paper strongly suggest that the replicase complex nsp3gene is the main pathogenic determinant conferring the avirulentphenotype of A7(74) and provide a rare example of the presenceof an opal termination codon in one alphavirus strain but notin another. In contrast, the structural genes of A7(74) do notseem to limit viralreplication.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell cultures. Cerebellar granule neurons were isolated from 7-day-old Harlan Spraque Dawley rats (Harlan Laboratories) as described before(5). Briefly, the pups were decapitated, and the cerebellawere removed into phosphate-buffered saline (PBS). The meningeswere carefully removed, and the tissue was chopped with a razorblade, trypsinized, and subsequently resuspended by tituratingin DNase containing trypsin inhibitor to separate the cells. Thecells were cultured in Eagle's minimal essential medium (MEM;Gibco-BRL) containing 2 mM glutamine, 50 U of penicillin per ml,and 50 µg of streptomycin per ml, supplemented with 10% (vol/vol)fetal calf serum (Gibco), 20 mM KCl, and 30 mM glucose. After1 day in culture, the medium was replaced with fresh medium containing10 µM arabinocytidine (Sigma) to inhibit the replication of nonneuronalcells, thus maintaining the purity of the culture. The cultureswere maintained at 37°C in a humidified atmosphere of 5% CO₂-95%air on poly-L-lysine-coated cell culture plates untilinfected.

BHK-21 cells (American Type Culture Collection) were maintained in BHK-21 medium (Glasgow-MEM) supplemented with 5% fetalcalf serum, 5% tryptose phosphate, 2 mM glutamine, and 10 mg ofgentamicin perliter.

MBA-13 cells were obtained through transformation by Epstein-Barr virus of mouse brain cells and possess the antigenic propertiesof oligodendrocytes (unpublished data). The cells were maintainedin Eagle's MEM supplemented with 5% fetal calf serum and 10 mgof gentamicin perliter.

Virus strains and passage histories. The SFV4 clone, a prototype derivative, was obtained by in vitro transcription of the full-length cDNA clone pSP6-SFV4, kindlydonated by P. Liljeström (Stockholm, Sweden). The A7(74) strainused for molecular cloning in the present study was originallyderived by Bradish et al. (4) from strain AR2066 through sevenpassages in neonatal mouse brain and two plaque purifications.We obtained this strain from H. E. Webb (London, United Kingdom),and it has since then been passaged several times in MBA-13 cellsand subsequently plaque-purified three times on the same cellsfor later molecular analyses and construction of the full-lengthgenome. The CA7 strain analyzed previously by Tarbatt et al. (46)was separated from the Bradish isolate after the initial sevenpassages in mouse brain (4) and passaged once more in mousebrain before three plaque-purifications and five or fewer passagesin BHK cells (G. Atkins, personalcommunication).

Sequence analysis. Sequence analysis of the recombinant A7(74), named rA774, and SFV4 nsp region genes was performed with a Perkin-Elmer ABIPrism automatic sequencer, model377.

Construction of full-length and chimeric RNA expression plasmids. The chimeric plasmids and viruses obtained are listed in Fig. 1. The validity of the intermediate plasmids was confirmed byrestriction fragment analysis or sequencing. The cDNA of the A7(74)nsp region was obtained by PCR following reverse transcriptionof the purified viral RNA (Ultraspec; Biotecx Laboratories). Theprimers were designed on the basis of the SFV prototype (44)sequence. Overlapping PCR fragments were cloned in the pGEM-Tvector (Promega) to produce intermediate plasmids. For constructionof the structural (str) region, cDNA was obtained from a lambdaphage cDNA library used recently for sequencing (34, 35).

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FIG. 1. Schematic illustration of the full-length SFV cDNA constructs used as a source for infectious RNA. Solid bars indicate SFV4 cDNA, and open bars represent the A7(74) genome. The pGEM1-derived vector (24) is not shown. The 21-nt deletion in prA774 alters the numbering of nucleotides with regard to SFV4. SFV4-specific nucleotide position numbers are given in italics. The 3' NTR of SFV4 is 334 nt shorter than that of rA774 (34). prA774 is the cDNA clone of A7(74). prA774-V4nstr was obtained by combining the 5'NTR and nonstructural genes of SFV4 with the structural genes and 3'NTR of rA774. prA774-V4str is reciprocal to prA774-V4nstr. In prA774-V4nsp12, a fragment containing the 5' NTR, nsp1, and nsp2 of SFV4 was introduced into prA774, and similarly, in prA774-V4nsp34 and prA774-V4nsp3, the indicated genes were used to replace the corresponding regions in rA774. In prA774-V4del, a short fragment of SFV4 nsp3 containing the 21 nt deleted in rA774 has been inserted into the corresponding region of rA774. prA774-arg differs from rA774 only by having an arginine codon at the opal position. pV4-opal is identical to SFV4 except that the arginine has been mutated to opal.

To exactly link the rA774 5'-nontranslated region (5'NTR) cDNA with the promoter region of pSP6-SFV4, site-directed mutagenesiswas used. The 5'NTR of rA774 was first cloned into the NcoI siteat the vector junction region of pSP6-SFV3 (24), followed byremoval of the two C residues from the NcoI site by site-directedmutagenesis to obtain a transcriptionally more active construct(24). The procedure for connecting the rA774 3'NTR to the pSP6-SFV4vector has been described previously (36).

To link the nsp3 gene with nsp4 in the prA774-V4nsp3 construct, PCR was used to create a BstZI site at nucleotide (nt) 5524.pV4-opal, a derivative of pSP6-SFV4 containing an arginine-to-opal(CGA to UGA) mutation (nt 5519), and a reciprocal, rA774-arg,with an arginine codon at the opal position in rA774, were obtainedby in vitro mutagenesis (17). DNA sequence analysis was usedto verify the sequences of the mutantclones.

Virus production. Intact full-length cDNA clones were transcribed in vitro using reagents from Boehringer, and the RNA transcripts were electroporatedinto BHK-21 cells (Bio-Rad gene pulser) (24). For large-scalepreparation, viruses obtained from the primary cultures were propagatedin MBA-13 cells in roller bottles as described previously (35).

Treatment of mice. Four- to seven-week-old, specific-pathogen-free female BALB/c AnNHsd mice (Harlan Laboratories) were used throughout thisstudy and treated and housed at the animal facility of the Universityof Turku in accordance with the guidelines of the University EthicsCommittee.

For mortality studies, 15 to 20 mice were inoculated intraperitoneally (i.p.) with 10⁶ PFU of virus in 100 µl of PBS and observed daily for 20 days.Another group of 16 mice were infected as above for virus titrationand immunohistochemistry. Two mice were sampled daily for a periodof 8 days. Mice were anaesthesized with CO₂, and blood was collectedwith a heparinized pipette from the right ventricle, after whichthe mice were perfused with cold PBS. Brains and spinal cordswere removed, and the brains were divided sagittally. One halfof the brain and the spinal cord were immersed in 4% PBS-Formalinfor at least 24 h before being embedded in paraffin wax. Deparaffinizedsections (4 µm thick) were stained for SFV antigens with a polyclonalA7(74)-specific antibody and the avidin-biotin-peroxidase detectionmethod (Vectastain ABC kit; Vector Laboratories). The SFV-specificantibody was produced in a rabbit immunized with purified, inactivatedA7(74). Appropriate antigen-negative controls were obtained frommice inoculated with PBS, while negative staining controls wereprovided by processing SFV4-positive samples and omitting theprimary antibody. The other half of the brain was taken in PBSand homogenized. The homogenate was centrifuged, and the supernatantwas used for virus titration. The blood samples were stored at4°C until centrifuged at low speed and diluted 1:10 in PBS. Virustiters were obtained by analyzing plaque formation in MBA-13 cellsas described previously (35).

Virus RNA detection. Confluent BHK-21 cell layers and 72-h-cultured primary rat cerebellar granule neurons on 12-well dishes were infected withvirus at a multiplicity of infection (MOI) of 20 in 0.2-ml Glasgow-MEMand conditioned medium (MEM), respectively, and incubated at 37°Cfor 1 h. The medium was replaced with 0.3 ml of warm medium containing1 µg of actinomycin D per ml for 2 h at 37°C and incubated fora further 3 h in the same conditions except for the addition of20 µCi of [5,6-³H]uridine (Amersham) per ml. Wells were washed twice with ice-coldserum-free medium and incubated on ice twice with 1 ml of 10%trichloroacetic acid (TCA) for at least 5 min. TCA precipitateswere solubilized in 1 ml of 10% sodium dodecyl sulfate (SDS).One fifth was mixed with 3 ml of scintillation cocktail (OptiPhaseHiSafe3), and the activity was determined with a liquid scintillationcounter (1216 Rackbeta; Wallac, Turku,Finland).

Western analysis. Rat cerebellar granule neurons cultured for 72 h were infected on 12-well plates at an MOI of 10 in 0.2 ml of conditionedmedium (MEM). After 0.5 h at 37°C, the medium was replaced with0.8 ml of conditioned medium. The cells were incubated at 37°C,and at 0, 8, and 24 h, samples were collected by removal of mediumand addition of 100 µl of Laemmli sample buffer. The samples weresonicated briefly with a needle sonicator, and the proteins wereseparated by SDS-12% polyacrylamide gel electrophoresis (SDS-PAGE).One tenth of the sample was run and stained with Coomassie tocontrol for the amount of protein, while an identical gel wasblotted on nitrocellulose (Schleicher & Schuell) with a HoeferSemi-Phor blotter (Hoefer Scientific Instruments), 0.8 mA/cm² for 30 min at room temperature. The filter was blocked in PBS-0.4%Tween containing 10% dry milk and incubated subsequently in thepresence of SFV-specific rabbit serum (1:6,000 dilution) in PBS-0.4%Tween containing 3% dry milk and peroxidase-conjugated goat anti-rabbitantibody for 1 h at room temperature. The filter was developedusing enhanced chemiluminescence (ECL) reagents from Amersham.Exposure times on Kodak X-OMAT AR film varied between 1 and 3min.

Confluent BHK-21 cells in 60-mm plates and 72-h-cultured rat cerebellar granule neurons on 35-mm plates were infected at anMOI of 10 with SFV chimeras in Glasgow-MEM and conditioned MEM,respectively, at 37°C for 30 min. Virus was removed, and afterreplacement of medium, incubation was continued for 3 h at 37°C.The medium was then removed, and the cells were suspended in 0.2or 0.1 ml of reducing sample buffer and sonicated briefly to shearthe DNA. Samples of 3.5 to 20 µl were run on SDS-10 to 12% PAGEand blotted onto a nitrocellulose membrane, and nsP3 and nsP4were detected with monospecific polyclonal antibodies made inrabbits (generously provided by L. Kääriäinen, Helsinki, Finland)by the ECL method(Amersham).

Nucleotide sequence accession numbers. The EMBL, GenBank, and DDBJ accession numbers for rA774 are: 5'NTR/nsp1/2, Y17207; nsp3, Y12518; nsp4, Y14761; capsid,X78109; E3, X78110; E2, X78111; 6K, X78112; E1, X74425;3'NTR, X74423. The SFV4 sequence number is AJ251359, andthe SFV prototype number is X04129.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Sequence analysis. Given the differences in the pathogenesis of rA774 and SFV4, we sequenced their entire nsp regions. Comparisons were madebetween these viruses and with CA7 (46), another attenuatedstrain of SFV which originates from the same isolate of virusesas A7(74) (4) (see Materials and Methods). For nsp1, 99.4 and98.1% nucleotide identity was observed compared with CA7 and SFV4,respectively, while the deduced amino acid sequences differedat five and six residues, respectively (Table 1). The nsp2 ofrA774 shows 98.5 and 98.1% identity to CA7 and SFV4, respectively,which predicts 20 and 4 amino acid differences,respectively.

In nsp3 of rA774, an in-frame deletion of 21 nt was detected at nt 5253 to 5273, abolishing seven amino acid residues (GIADLAA),which was retained in both SFV4 and CA7. The deletion site wasflanked on both sides by the motif 5'-GTGCACCCTGAACCCGCAG-3',present at this position in all three SFV strains. We showed byreverse transcription-PCR that the viral RNA species with thedeletion was the only RNA present in our original A7(74) virusstock. Sequence analysis further revealed an opal (UGA) terminationcodon in rA774 nsp3 at nt 5498, close to the nsp3-nsp4 junction,which was rather unexpected, as SFV4 and CA7 (46) both displayan arginine codon at the equivalent position. On the other hand,in several other alphaviruses, such as SIN, Middelburg virus (43),Ross River virus (42), and Venezuelan (16) and western andeastern (48) equine encephalitis viruses, an opal codon hasbeen found. The presence of the opal codon in the parental rA774was confirmed by sequencing three independent PCR clones obtainedfrom our original plaque-purified virus, and it could also beshown in the stock virus. Ignoring the 21-nt deletion, the nsp3gene of rA774 displayed 97.4 and 96.6% nucleotide identity withCA7 and SFV4, respectively, the mutations predicting 12 and 9amino acid changes, respectively (Table 1). The nsp4 gene ofrA774 exhibited 99.1 and 97.4% nucleotide identity with CA7 andSFV4, respectively, with the deduced amino acid sequences differingby only two amino acids in both (Table 1). Interestingly, inboth rA774 and CA7 (46), there was an adenine residue in nsp4(nt 7350 and 7371, respectively) immediately preceding the transcriptionstart site of 26S RNA, while SFV4 had a guanidine at this site(44). As this could have been critical for transcription efficiency,we replaced in rA774 the whole 26S RNA-encoding region, includingthe preceding 28 nt, with the equivalent SFV4 sequence. The recombinantdid not, however, display increased virulence (not shown). TheNTR between nsp4 and the capsid gene was identical in all threevirus strains.

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TABLE 1. Nucleotide substitutions in SFV nonstructural protein genes resulting in amino acid changes^a

A7(74) genome-length clone. The A7(74) virus is avirulent for adult mice but lethal for neonatal mice, whereas SFV4 is lethal for mice of all ages (8,27). It has been suggested that virulent strains reach a criticalthreshold titer in the central nervous system (CNS), leading toneuronal damage by either necrosis or apoptosis (10, 37).Virus chimeras have proven a powerful tool in identification ofpathogenic sites of viral genomes (32, 35). In order to facilitatethe construction of recombinant SFV for identification of genomeloci involved in attenuation of A7(74), a full-length cDNA ofA7(74) was synthesized and used to replace the prototype SFV insertin the pSP6-SFV4 plasmid (24). This plasmid, prA774, gave riseto rA774 virus after transcription with SP6 RNA polymerase (seeMaterials and Methods). rA774 replicated to comparable titersin mouse brain with the plaque-purified A7(74) (Fig. 2), althoughsomewhat lower titers were measured in the blood at days 1 and2. At day 3 the values in blood reached comparable levels in bothstrains (Fig. 2), and no virus could be detected in the samplesat 4 days postinfection or later. When administered i.p. (10⁶ PFU), rA774 was asymptomatic for adult BALB/c mice (Fig. 3),except that 1 mouse out of 20 showed opticus neuritis and anotherhad slight, transient hind limb paralysis. For neonatal mice,rA774 was lethal (unpublished results). In BHK-21 cells and culturedrat cerebellar granule neurons, the rA774 virus displayed a phenotypesimilar to that of the parental A7(74) (see below). The vehiclesprA774 and pSP6-SFV4 (24) were then used to construct a panelof recombinant viral RNA expression plasmids which, upon in vitrotranscription and transfection of mammalian cells, produced acollection of virus chimeras (Fig. 1).

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FIG. 2. Virus titers in the blood and brain of mice infected with SFV. Adult BALB/c mice were infected i.p. with 10⁶ PFU of virus in 100 µl of PBS. Serum and brains from two mice were taken each day. Each bar represents an individual animal. Stars indicate animals with titers under the detection limit (50 PFU/ml or 200 PFU/g). Note that the high titers at day 7 for both V4-opal-infected mice represent reversion of the mutants.

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FIG. 3. Kinetics of mortality in SFV infection. Four- to seven-week-old female BALB/c AnNHsd mice were infected i.p. with 10⁶ PFU of virus in 100 µl of PBS. The star indicates a V4-opal-infected mouse with irreversible hind limb paralysis that was sacrificed for histological analysis on day 13.

A7(74) replicase complex mediates attenuation. For the localization of virulence determinants, we first analyzed the function of the SFV4 replicase complex attached to thecomplete set of rA774 capsid and envelope glycoproteins includingthe 3'NTR, which differs from SFV4 in that it contains a 101-ntinsertion as well as a repeated motif (34). For this purposewe constructed a chimeric rA774-V4nstr virus (Fig. 1), which expressedthe nonstructural proteins of SFV4 and the proteins encoded bythe subgenomic 26S RNA of rA774. rA774-V4nstr was highly virulentupon intraperitoneal (i.p.) infection, with 10⁶ PFU of virus killing all of the 15 infected female mice (Fig.3) (15 of 15 male mice tested in parallel died as well [data notshown]), suggesting that the structural proteins of rA774 do notrestrict virus replication. rA774-V4nstr reached brain titersup to 7 × 10⁸ PFU/g, comparable to SFV4 (Fig. 2). This experiment also showedthat the viral NTRs are functionally compatible when originatingfrom avirulent and virulent strains. To analyze the reciprocalcase, rA774-V4str virus (Fig. 1) containing the rA774 replicasecomplex genes, including the 5'NTR combined with SFV4 structuralgenes was constructed, and the clone was shown to grow to onlymoderate titers (10⁴ to 10⁵ PFU/g) in murine brains, similar to rA774 (Fig. 2) in being asymptomaticfor adult animals (Fig. 3). This result confirmed that the avirulenceof A7(74) derives from the viral replicasecomplex.

Search for virulence loci within the replicase complex genes. Mutations introduced at multiple genome loci may interfere with the correct secondary structure of viral RNA or the functionalassembly of viral proteins, thus abolishing virulence, but transformingan avirulent virus to a virulent one requires introduction oftrue virulence determinants. We therefore sought to identify lociin the SFV4 nsp region which, when inserted into the avirulentrA774, would confer virulence. We first replaced rA774 nt 1 to3761, comprising the 5'NTR, nsp1, and nsp2, and nt 3761 to 7370,containing genes nsp3 and nsp4, with the corresponding segmentsof SFV4. The chimeras obtained were designated rA774-V4nsp12 andrA774-V4nsp34, respectively (Fig. 1). rA774-V4nsp12 showed increasedvirulence, killing 7 of 20 mice (Fig. 3) and causing paralyticsymptoms in an additional 6 animals, proving the involvement ofthis region in regulation of pathogenicity. rA774-V4nsp34 replicatedto high titers in the CNS of mice (Fig. 2) and killed 95% of theinfected animals (Fig. 3). As sequence analysis had revealed majormodifications in nsp3, the effect on virulence of this gene wasanalyzed next. A highly neurovirulent virus with a lethal phenotypecomparable to that of parental SFV4 and rA774-V4nstr was obtainedby replacement of the nsp3 gene in rA774 with the correspondingSFV4 nsp3 gene. The phenotype of this recombinant, designatedrA774-V4nsp3 (Fig. 1), was confirmed by histological analysis,and the virus showed wide spreading in the cortex and cerebellum,with Purkinje neurons and granule cells strongly affected (Fig.4C; also see below). In rA774-V4nsp3-infected BHK-21 cells, theamount of nsP4 was higher than that measured in the chimeras expressingrA774 nsP3 (see Fig. 6C). However, the corresponding viral RNAamounts in both BHK-21 cells and cultured neurons were clearlylower than the amounts produced by other virulent clones (seeFig. 6).

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FIG. 4. SFV polyclonal antibody-stained brain sections from mice infected i.p. with 10⁶ PFU of virus. (A) rA774 infection. Multiple small antigen-positive foci of virus are visible in the pons (P) and cerebellum (C) (arrows). Bar, 0.5 mm. (B) Widespread rA774-V4nstr infection of the pons (P), indicated with asterisks. Arrows, infected granule cells and cerebellar (C) Purkinje neurons with antigen-positive dendrites. Bar, 0.7 mm. (C) rA774-V4nsp3-infected areas of pons (P, asterisk) and cerebellum (C) with affected Purkinje cells, including dendrites (arrows). Bar, 0.6 mm. (D) rA774-V4del-infected cerebellum with a few viral foci (arrows). Bar, 0.6 mm. (E) Extensive rA774-arg invasion (asterisk) of the cerebral nucleus (putamen). Bar, 0.6 mm. (F) Widespread infection with V4-opal of brain hemisphere (arrows) of a mouse infected with the V4-opal construct which reverted to arginine. Bar, 0.7 mm.

Completion of the nsp3 deletion. To more closely analyze whether the deleted residues are responsible for the reduced CNS replication and pathogenicity ofrA774, the seven deleted amino acids (GIADLAA) in the nonconservedregion of nsP3 were reconstructed. Given that a membrane-bindingfunction has been ascribed to the alphavirus nsP3 protein, itwas possible that the absence of such a hydrophobic domain couldreduce its binding properties and thus could affect transcription.Reconstruction in rA774 of this deleted site with a 327-nt fragmentfrom SFV4 that restored the amino acid sequence resulted in recombinantrA774-V4del virus (Fig. 1). This chimera was, however, unableto replicate in mice to titers high enough to cause clinical symptoms(Fig. 2), and it could not be phenotypically distinguished fromthe parental rA774 virus or other avirulent clones (Fig. 3).

In vitro mutagenesis of the in-frame opal codon. In SIN, an opal termination codon in the nsp3 gene close to the nsp4 junction dramatically reduces the amount of nsP4 mRNA(25). In order to analyze the role of the opal codon in rA774replication, two mutant viruses were constructed. First, the opalcodon in rA774 was changed to an arginine (CGA) codon, and second,the arginine (amino acid 476) CGA (nt 5516) in SFV4 was mutatedto a UGA stop codon. The resulting viruses, rA774-arg and V4-opal,respectively (Fig. 1), were then tested in adult BALB/c mice.The rA774-arg clone with nonrestricted readthrough displayed markedlyincreased virulence compared to rA774, killing 1 of 20 mice (Fig.3) and causing paralysis in 5 of 20 mice, being, however, farless virulent than the parental SFV4 and the lethal rA774-V4nstror rA774-V4nsp3 chimeras. Upon i.p. infection with the V4-opalmutant, 3 mice out of 20 died (Fig. 3), and a fourth mouse showedhind limb paralysis. In another experiment, we isolated virusfrom the brains of 2 V4-opal-infected mice (total, 16) who weremoribund at day 7, which showed a high virus titer in the brain(Fig. 2) and a high virus load in the CNS (Fig. 4F) at the timeof sampling. We showed with RT-PCR and sequencing that in thesemice the opal codon had undergone mutation, giving rise to anarginine (CGA) codon in one and a tryptophan (UGG) codon in theother mouse, indicating that V4-opal is unstable and most probablyeven less virulent than what was indicated by the mortality numbers.The viruses in the brains of the affected mice in the mortalitystudy were not sequenced, but it is possible that reversion wasalso responsible for the reoccurrence of virulence in these. Thelate mean day of death (9.7) (Table 2) in V4-opal-infected miceprobably indicates slow evolution of revertants. Thus, the resultswith the V4-opal mutant suggested an important role for the opalcodon in regulation of virulence.

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TABLE 2. Mortality after SFV infection^a

The stability of the opal codon in A7(74) and rA774 might be explained by lack of replication advantage of any sense mutation,as observed for SIN, in which sense mutants of opal displayeda lower RNA synthesis rate than the opal (23). Although introductionof arginine at the opal site did not markedly increase lethality,the observed paralytic symptoms indicate a considerable increasein virulence, which suggests a significant role for opal as anattenuating factor inrA774.

Replication of virus in blood and brain. Generally, mice infected with SFV chimeras or mutants constructed in this study developed plasma viremia at day 1 postinfection(Fig. 2). No virus could be detected in the blood after 2 daysin rA774-V4str- or V4-opal-infected mice, whereas rA774 and rA774-V4nstrhad been cleared by day 4. In accordance with the mortality studies,the virulent clones SFV4, rA774-V4nstr, rA774-V4nsp34, and rA774-V4nsp3replicated to high titers in the brain (10⁸ to 10⁹ PFU/g of brain tissue), whereas the avirulent A7(74), rA774,rA774-V4str, rA774-arg, and rA774-V4del reached moderate values(10³ to 10⁷ PFU/g of brain tissue). We frequently observed no virus in thebrains of mice infected with rA774-V4str and V4-opal. In a recentstudy in our laboratory (36) and that of Grieder et al. (12),similar observations were made for alphavirus E2 in vitro mutants.This phenomenon could be explained, for example, by a reducedcapacity of the virus to migrate to and/or penetrate the CNS,and indeed, infected mice lacking CNS pathology had developedserum antibody titers comparable to those measured in mice showingeffective virus dissemination in the brain (36). It is of interestthat while the majority of the V4-opal-infected mice displayedvirus titers in the brain lower than those of A7(74)-infectedmice, with little or no virus detected in histology, the two micedisplaying high virus titers (10⁸ to 10⁹ PFU/g) (see above) at day 7 were those infected with arginineand tryptophanrevertants.

Histochemical analysis. In general, the degree of virulence of the SFV chimeras and mutants, expressed as percent survival (Fig. 3), correlated wellwith the spreading and distribution of the virus within the CNS,as demonstrated by the histochemical analysis (Fig. 4). Like theplaque-purified parental A7(74), the rA774 clone was unable toefficiently disseminate in brain tissue, forming only a few scatteredfoci, mainly in the perivascular areas (Fig. 4A). In contrast,the virulent rA774-V4nstr virus effectively spread along the cerebellarPurkinje cell dendrites, occupying practically the entire brain(Fig. 4B), similar to SFV4 (41). Of mice infected with the reciprocalrA774-V4str, only one was virus antigen positive (not shown).The rA774-V4nsp3 chimera showed no restriction in disseminationwithin the spinal cord and brain, and abundant virus was foundin the cerebellum, cortex, and pons areas (Fig. 4C). In contrast,only a few foci were detected in the brains of rA774-V4del-infectedanimals (Fig. 4D), while in rA774-arg-infected brains (Fig. 4E),the virus load was markedly higher, indicating improvedspread.

In V4-opal infection, virus spread in the neural tissue of the clinically asymptomatic animals was generally extremely limited(not shown), comparable to rA774, except for one asymptomaticmouse which at day 7 postinfection displayed a high virus loadin the cortex and pons as well as in the periventricular areasbut with no virus detected in the cerebellum (not shown). Bothmoribund mice sampled in this group were shown to be infectedwith opal revertants, and they displayed extensive virus spreading.The arginine revertant shown in Fig. 4F invaded the cortex andcerebrum. We also undertook histological studies on one affectedmouse from the mortality study group, indicated with an asteriskin Fig. 3, which displayed left hind limb paralysis although otherwiseclinically healthy. Severe myelin destruction was manifested,with numerous macrophages in the spinal cord, both phenomena similarto those observed during Wallerian degeneration (notshown).

Analysis of RNA and protein synthesis in cultured cells. Viral RNA production was measured by infecting confluent monolayers of cultured BHK-21 cells and 72-h-cultured primary ratcerebellar granule neurons at an MOI of 20 with virus chimeras.[5,6-³H]uridine was used to label the RNA synthesized in the presenceof actinomycin D (see Materials and Methods), and TCA-precipitatedtotal RNA was analyzed by liquid scintillation counting. Highrelative RNA amounts were synthesized in BHK-21 cells infectedwith virulent SFV4, rA774-V4nsp12, and rA774-V4nstr, while avirulentA7(74), rA774, and rA774-V4del showed decreased expression (Fig.5). However, elevated levels of viral RNA were also observed forthe avirulent rA774-V4str and V4-opal mutants, while unexpectedlylow amounts were synthesized by the virulent rA774-V4nsp3, whichon the other hand produced nsP3 and nsP4 proteins in quantitiescomparable to those produced by SFV4 and rA774-V4nstr (see Fig.6C). Moderate levels of RNA expression were obtained with therA774-arg mutant. In neurons, only virulent SFV4 and rA774-V4nstrinfections produced viral RNA amounts clearly above those seenin infections with the avirulent chimeras. These results showthat virulence does not in all instances correlate with the amountof viral RNA.

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FIG. 5. Viral RNA synthesis during early infection measured by scintillation counting. BHK-21 monolayers (solid bars) and 72-h-cultured rat cerebellar granule neurons (open bars) were infected with parental strains and recombinants at 20 PFU per cell. [³H]uridine was added at 3 h postinfection, and cells were lysed 3 h later in 10% SDS. Actinomycin D was used to inhibit cellular RNA synthesis. Control cells (C) were uninfected. The star indicates a value below 500 cpm.

Given the phenotypic differences between the distinct SFV nsp chimeras, we sought to study the synthesis of nsP3 and nsP4as well as the expression of the viral structural proteins duringinfection. Generally, the expression of the nonstructural proteinsby the virus chimera in cultured rat cerebellar neurons was muchlower than that measured in BHK-21 cells. As the amounts of nsP4were extremely low and the antibody showed binding to cellularproteins, the estimation of nsP4 amounts was somewhat hampered.In cultured neurons, the virulent chimeras produced higher amountsof nsP3 and nsP4 than the avirulent clones, as shown by immunodetection(Fig. 6A), which is in accordance with the titers obtained inmouse brains (Fig. 2). However, plaque-purified A7(74) expressednsP3 amounts similar to those expressed by rA774-V4nsp12 and rA774-V4nsp3.The same was generally true for BHK-21 cells, although here V4-opalalso showed elevated levels (Fig. 6C). These results show thatvirulence does not in all instances correlate with protein amounts,and it is possible that, e.g., temporal differences in the viralprotein levels are of importance. There was a tendency, however,for the chimeras with an arginine codon at the opal position innsp3, including the avirulent rA774-arg mutant, to express higheramounts of both nsP34 and nsP4 in neurons (Fig. 6A). In BHK-21cells, SFV4, rA774-V4nstr, and rA774-V4nsp3 showed clearly increasednsP4 expression compared with the apathogenic virus chimeras.In cultured rat neurons, the expression levels of the viral structuralproteins were similar at 8 h postinfection, but differences becamemore pronounced at 24 h after infection, SFV4 and rA774-V4nstrshowing clearly higher relative amounts compared with virulentrA774-V4nsp3 and rA774-V4nsp12 and the apathogenic chimeras (Fig.6B).

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FIG. 6. Expression of viral proteins in cell cultures infected with parental and chimeric SFV. At given time points, the cells were lysed in Laemmli sample buffer and sonicated briefly to shear DNA prior to SDS-PAGE. The proteins were blotted onto nitrocellulose and visualized with specific antibody and peroxidase ECL detection. (A) Production of the nonstructural proteins nsP3 and nsP4 was measured 3.5 h after infection of 72-h-cultured rat cerebellar granule neurons (10 PFU/cell). Polyclonal monospecific antibodies (provided by L. Kääriäinen) were used in detection. (B) Synthesis of capsid protein and E1 and E2 envelope glycoproteins (visible as one overlapping band) in cultured rat cerebellar granule neurons. Samples were taken at the indicated time points postinfection. Polyclonal SFV-specific rabbit antibody was used for detection. (C) Production of the nonstructural proteins nsP3 and nsP4 in SFV-infected monolayers of BHK-21 cells was measured as described above for neurons. The applied amounts of total protein were highly similar, as confirmed by Coomassie staining (not shown).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In several alphaviruses, mutations in the glycoprotein genes alter virulence (6, 11, 47), and mutations in both E2and E1 may have a synergistic effect (32). Alterations in E2protein may affect SFV virulence, as shown by our recent analysis(35), in which an SFV chimera (CME2) carrying seven of a totalof eight A7(74) E2 amino acid mutations was highly attenuated,and by two other studies, in which single E2 amino acid residuescontributing to attenuation were identified (9, 36). TheE2 gene does not, however, represent a natural avirulence determinantof A7(74) as demonstrated by this study, showing that the entityof the structural protein-encoding genes of rA774 in associationwith the SFV4 replicase complex in the rA774-V4nstr chimeric virusare capable of composing a highly virulent virus. The avirulentphenotype of the SFV4-derived CME2 (35) could derive from afunctional failure of the E1-E2 complex with E2 originating fromrA774. Amino acid mutations in this chimeric spike complex couldprevent proper structureformation.

The complete nonstructural genome sequence of rA774 determined in this study revealed a large number of nucleotide mutationscompared with SFV4, which often led to changes in the predictedamino acid sequence. The most notable differences were those detectedin the nsp3 gene of rA774, of which the in-frame deletion of 21nt in the nonconserved gene region abolished seven amino acidresidues, five of which are hydrophobic. Although the role andinteractions of nsP3 in alphavirus replication remain unclear,its role as a docking protein stabilizing the active replicasecomplex on cytopathic vacuoles has been suggested, and it hasbeen shown to accumulate on cellular vacuole surfaces (28, 29).Thus, it was possible that this particular domain with the deletioncould be involved in forming the putative contact surface forcytopathic vacuoles, and hence changes at this site that reducehydrophobicity might also reduce the amount of vesicle-bound nsP3,thus lowering RNA synthesis efficiency. However, the fact thatintroduction into rA774 of the deleted residues comprising theheptapeptide GIADLAA did not increase virulence excluded thispossibility and rather confirmed previous observations that thenonconserved C-terminal domain of alphavirus nsP3 allows remarkablechanges in both length and sequence without affecting the phenotype(20).

The opal codon in nsp3 of rA774 was an unexpected finding, because the SFV4 and CA7 strains (46) both express an argininecodon at this site. Although most alphaviruses express an opalcodon (16, 42, 43, 48), its significance in the regulationof alphavirus pathogenesis remains elusive. Such human pathogensas the Venezuelan (16) and eastern (48) encephalitis viruses,which cause severe disease, contain an opal codon at this position,indicating its selective advantage and stability. In vitro, usingSIN RNA, readthrough of the opal codon has been estimated to occurwith about 20% of the efficiency of that of a sense mutant (7),and in another study, mutants with sense replacements showed adelay in the appearance of nsP3 and reduced levels of this protein(23). Also, in the same report, in cell cultures SIN RNA synthesiswas rather reduced in mutants with in vitro replacement of theopal with different sense codons. This was ascribed to the increasedturnover rate of the nsP4protein.

The present study shows that in SFV, the opal site in nsp3 affects virus pathogenesis in mice. The introduction of an opalcodon dramatically attenuated SFV4, making it nearly avirulentfor adult mice, while replacement of the opal codon in rA774 withan arginine clearly increased pathogenicity even if it was notsufficient to restore full virulence. While SFV4, rA774-V4nstr,and rA774-V4nsp3 all caused neurological symptoms within a shortperiod before the mice succumbed, the rA774-arg mutant, whichkilled only one mouse, nevertheless frequently caused transientparalysis and limb weakness, thus exhibiting a medium degree ofvirulence not observed forrA774.

Generally, the viral RNA synthesis rate correlated well with the degree of virulence, but the increased pathogenicity maynot always necessitate an increase in RNA synthesis, as indicatedby the fact that the viral RNA levels in rA774-V4nsp3-infectedneurons were much lower than those obtained with mutants of similarvirulence. Also, the levels of RNA in rA774-arg-infected hamstercells were comparable to those found in asymptomatic A7(74) infection,but much lower than those produced by the completely avirulentrA774-V4str chimera. It is interesting that in neurons, the naturalhost cells of SFV, rA774-V4str produced much lower amounts ofRNA than it did in hamster kidney cells, indicating cell type-specificregulation and control aswell.

Virulence correlated poorly with the levels of the viral structural proteins in neuronal cell cultures, as of the pathogenicclones, only SFV4 and rA774-V4nstr produced remarkably increasedamounts, while the lethal rA774-V4nsp3 showed glycoprotein levelssimilar to those with A7(74) (Fig. 6B). In contrast, expressionof nsP4 in hamster cells was in accordance with the degree ofpathogenicity, with levels clearly elevated for the lethal mutantsand significantly increased for rA774-arg, which had moderatevirulence (Fig. 6C).

As demonstrated by the pathogenicity tests using the rA774-V4nsp34 and rA774-V4nsp3 chimeras, nsP3 of SFV4 alone was sufficientto mediate lethal neurovirulence, showing that the two amino aciddifferences found in nsP4 do not significantly alter virus phenotype.However, it cannot be excluded that if used to replace the correspondingrA774 gene, nsp4 of SFV4 could alter virulence. Like the nsP4of SFV4 and other alphaviruses, the nsP4 of rA774 displayed anN-terminal tyrosine, the only amino acid residue at this sitethat allows full replication efficiency (39). The significantlyincreased virulence observed for the rA774-V4nsp12 chimera comparedwith parental rA774 indicated that the SFV4 nsp12 locus partiallycompensates for the attenuation deriving from nsp3. Although thecontribution to pathogenicity of the nsp1 gene was not separatelytested, it probably is involved, because in a reciprocal analysis,an SFV4 derivative expressing nsp1 of rA774 displayed a remarkablyattenuated phenotype in adult mice (unpublished data). This doesnot, however, exclude the involvement of nsp2 as well, becausea few amino acid mutations were found in this region (Table 1).These results fit into the present view of alphavirus replicationthat nsP1 participates in forming a vacuole-docking unit of thereplicase complex together with nsP3 (30), and for such vacuoles,the membrane affinity of the replicase multiprotein complex canbe assumed to determine its surface concentration, a parameterpotentially affecting virus replicationefficiency.

Previous analyses of the structural genome of the SFV derivatives rA774 (34, 35) and CA7 (9) suggested that the twostrains are nearly identical, as only four amino acid differenceswere detected. The present analysis of the nonstructural genome,however, clearly established that these are two essentially differentSFV strains, although they both derive from the original Bradishisolate (4). The nsp regions of these two strains showed majordifferences in the sequence per se; also, whereas in rA774 theavirulence was primarily mediated by nsp3, with less pronouncedcontributions by nsp1 or nsp2 and with the structural genome beingfully functional, in CA7 the attenuating domains were found distributedin both structural and nonstructural parts of the genome (46).However, in contrast to rA774, the nsp3-nsp4 region of CA7 wasnot found to contain major attenuating determinants. Hence, thesestrains should not be considered equivalent, as this might producecontradictory results because the causative mutations reside instructures with fundamentally different functions in viralreplication.

Our analysis has shown that the genetic loci responsible for the natural avirulence of SFV A7(74) reside entirely in the nonstructuralgenome and that they mainly derive from changes in the nsp3 gene,with a significant contribution by the opal mutation, not foundin SFV4, whereas the 21-nt deletion at the nonconserved carboxyterminus does not affect virus phenotype. Further analyses arerequired to assess the role of the single nsP3 amino acid mutationsin the regulation of SFVreplication.

	ACKNOWLEDGMENTS

This work was supported by the Sigrid Juselius Foundation, the Finnish MS-Foundation, and the Åbo AkademiUniversity.

We thank Michael Courtney for help with the rat cerebellar granule neurons and for revising the English and Petri Auvinenfor critical reading of the manuscript. We also thank Seija Lindqvistfor excellent animal care, Marja Aaltonen for help in plaque titration,Hanna Laurén for prA774-V4nsp34 construction, and Jaakko Liippofor experienced preparation of the photographs. We are gratefulto Leevi Kääriäinen for providing the nsP antibodies. Thanksare also due to Gregory Atkins and Harry Kujari for helpfuldiscussions.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Pharmacy, Åbo Akademi University, FIN-20520 Turku, Finland.Phone: 358-2-2154141. Fax: 358-2-2154745. E-mail: minna.tuittila{at}ra.abo.fi.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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