Pathogenesis of Chimeric MHV4/MHV-A59 Recombinant Viruses: the Murine Coronavirus Spike Protein Is a Major Determinant of Neurovirulence

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Journal of Virology, September 1999, p. 7752-7760, Vol. 73, No. 9
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Pathogenesis of Chimeric MHV4/MHV-A59 Recombinant Viruses: the Murine Coronavirus Spike Protein Is a Major Determinant of Neurovirulence

Joanna J. Phillips,¹ Ming Ming Chua,¹ Ehud Lavi,² and Susan R. Weiss¹^,^*

Departments of Microbiology¹ and Pathology,² University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104-6076

Received 2 April 1999/Accepted 28 May 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The mouse hepatitis virus (MHV) spike glycoprotein, S, has been implicated as a major determinant of viral pathogenesis. Inthe absence of a full-length molecular clone, however, it hasbeen difficult to address the role of individual viral genes inpathogenesis. By using targeted RNA recombination to introducethe S gene of MHV4, a highly neurovirulent strain, into the genomeof MHV-A59, a mildly neurovirulent strain, we have been able todirectly address the role of the S gene in neurovirulence. Incell culture, the recombinants containing the MHV4 S gene, S4R22and S4R21, exhibited a small-plaque phenotype and replicated tolow levels, similar to wild-type MHV4. Intracranial inoculationof C57BL/6 mice with S4R22 and S4R21 revealed a marked alterationin pathogenesis. Relative to wild-type control recombinant viruses(wtR13 and wtR9), containing the MHV-A59 S gene, the MHV4 S generecombinants exhibited a dramatic increase in virulence and anincrease in both viral antigen staining and inflammation in thecentral nervous system. There was not, however, an increase inthe level of viral replication in the brain. These studies demonstratethat the MHV4 S gene alone is sufficient to confer a highly neurovirulentphenotype to a recombinant virus deriving the remainder of itsgenome from a mildly neurovirulent virus, MHV-A59. This definitivelyconfirms previous findings, suggesting that the spike is a majordeterminant ofpathogenesis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The Coronaviridae family of viruses is studied widely for its ability to generate diseases in a number of different animalhosts. Mouse hepatitis virus (MHV), a member of this family, providesa useful model system for studying both acute and chronic virus-inducedneurologic disease. Intracranial or intranasal inoculation ofsusceptible mice with neurotropic strains of MHV can result ina range of outcomes from acute encephalomyelitis to chronic demyelinatingdisease (1, 24). The outcome of infection is determined bya number of factors, including the viral strain, dose, route ofinoculation, host strain, age, and immune status (9). The roleof the viral strain in determining the severity of the acute diseaseis well established, but the viral determinants which explainthese differences are not known. Two strains which differ markedlyin their neurovirulence are MHV4 and MHV-A59. Infection of weanlingmice with low doses of MHV type 4 (MHV4, a strain JHM isolate),a highly neurovirulent strain, produces a severe and often fatalencephalitis (10), while much higher doses of MHV-A59, a mildlyneurovirulent strain, are required to produce a mild encephalitis(28, 29).

The lack of an infectious molecular clone of MHV has limited the study of viral determinants of pathogenesis to the comparisonof different strains and mutant viruses. From these comparisons,however, it has become evident that the MHV spike (S) glycoproteinplays a key role in pathogenesis. The importance of the S proteinin pathogenesis is consistent with its biologic function in bothviral entry and viral spread (8, 46). When expressed on thevirion envelope, S binds to the cellular receptor and inducesthe fusion of viral and cell membranes during viral entry. Subsequentto infection, S protein expressed on the plasma membrane of infectedcells induces cell-cell fusion. S also plays a role in the immuneresponse to viral infection, as a target for neutralizing antibodies(8) and as an inducer of a cell-mediated immunity (4, 7).

The S glycoprotein, arranged in a homo-oligomeric structure on the virion surface, forms the characteristic spikes protrudingfrom the virion envelope. For most strains, the S protein is cleavedposttranslationally into an amino-terminal (S1) and a carboxy-terminal(S2) subunit (16, 44). S1 is believed to make up the globularhead of the spike and has been demonstrated to exhibit a receptor-bindingactivity (12, 26). The S2 subunit, containing a transmembranedomain and two heptad repeat regions, is believed to form thestalk portion of the spike and to mediate membrane fusion (12,34).

From the study of numerous variant viruses, selected for resistance to neutralizing monoclonal antibodies, an associationhas been made between various mutations or deletions in S andneuroattenuation (10, 15, 19, 37, 45). Interestingly,many of these viruses display mutations or deletions in a regionof S1 termed the hypervariable region (HVR), or in and aroundthe heptad repeat regions of S2. In general, it is not known howmutations in the HVR or in S2 could affect neurovirulence, butit has been suggested that they may affect fusogenicity, cytotoxicity,viral spread, or receptor binding (13, 17, 40).

Until recently, the technology to introduce specific mutations into the MHV genome was not available, and thus pathogenesisstudies had to rely on associations drawn from the comparisonof nonisogenic variant viruses. With the development of targetedrecombination, the 3' end of the MHV genome containing the structuralgenes has been made available for genetic analysis (14, 31).Using this technique, we have generated isogenic recombinant virusesthat contain either the S gene of the highly neurovirulent MHV4or the S gene of the mildly neurovirulent MHV-A59. With thesepairs of recombinant viruses we have been able to directly addressthe role of the S gene in neurovirulence. Recombinant viruses,containing the MHV4 S gene, displayed a dramatic increase in virulence,while control recombinant viruses, containing the wild-type MHV-A59S gene, displayed a pathogenesis similar to that of wild-typeMHV-A59. This increase in virulence was associated with an increasein viral antigen expression and inflammation, but not in the extentof viral replication in the central nervous system(CNS).

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Virus and cells. MHV-A59 was obtained from Lawrence Sturman (Albany, N.Y.). MHV4 was obtained from Michael J. Buchmeier (La Jolla, Calif.).Alb4 (obtained from Paul Masters, Albany, N.Y.) contains an 87-nucleotidedeletion (resulting in a 29-amino-acid in-frame deletion) in anonessential spacer region in the N (nucleocapsid) gene; it producessmall plaques at the nonpermissive temperature (39°C) and is thermolabile(25). Murine L2 cells and 17Cl-1 cells were maintained on plastictissue culture flasks in Dulbecco minimal essential medium (DMEM)with 10% fetal bovine serum (FBS). Spinner cultures of L2 cellswere maintained in Joklik minimal essential medium with 10% FBSat densities of between 2 × 10⁵ and 2 × 10⁶ cells perml.

Plasmids and PCR mutagenesis. The construction of pMH54 (obtained from Paul Masters) involved the extension of the pFV1 vector (14) to include the 3'1.1-kb of the hemagglutinin esterase gene of MHV-A59 (26a) (seeFig. 1). The inclusion of the 3' portion of the hemagglutininesterase gene in the pMH54 plasmid allowed us to select for viruseswhich had recombined 5' to the S gene, and thus contained theentire recombinant spike gene. The sequence of the S gene in pMH54is the same as that of wild-type MHV-A59 (23) except for theintroduction of AvrII and SbfI restriction sites. The AvrII sitewas created by introducing two silent mutations in codons 12 and13 of S. The SbfI site was generated in the intergenic regionbetween gene S and gene 4 by making three nucleotide substitutionsat 12, 15, and 17 bp past the S gene termination codon. The AvrII/SbfIsites allowed us to easily introduce different S genes into thebackground of pMH54 and to identify recombinant viruses containingfull-length recombinant spike genes. For RNA transcription, theplasmid was linearized just 3' to the poly(A) tail by digestionwith PacI.

The pGEM4Z plasmid containing the MHV4 S gene, pSwt (18), was obtained from Michael J. Buchmeier. To replace the MHV-A59S gene in pMH54 with the MHV4 S gene, we introduced the AvrIIand SbfI restriction sites into the MHV4 S gene. This was doneby PCR mutagenesis (22) with Vent polymerase and the primerslisted in Table 1. A restriction fragment containing the AvrIIsite (and a HindIII cloning site) was generated by amplificationwith primers JJ2 and A59-4. The 1,185-bp PCR fragment was gelpurified, digested with restriction enzymes HindIII and PflmI,and then cloned into the corresponding sites in pSwt. This clonewas designated pG-MHV4-S1, and the entire 728-bp fragment wassequenced. A restriction fragment containing the SbfI restrictionsite (and a BamHI cloning site) was also generated by amplificationwith primers wzl-15 and JJ3. The 875-bp PCR fragment was gel purified,digested with the restriction enzymes BsmI and BamHI, and thencloned into the corresponding sites in pG-MHV4-S1. This clonewas designated pG-MHV4-S2, and the entire 670-bp fragment wassequenced. The pG-MHV4-S2 plasmid was digested with restrictionenzymes AvrII and SbfI, and then cloned into the correspondingsites in pMH54. This clone was designated pMH54-S4, and sequencingconfirmed that no secondary site mutations had been introduced.

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TABLE 1. Primers used for mutagenesis of pSwt and for recombinant genome sequencing

Targeted RNA recombination and selection of recombinants. Targeted RNA recombination was carried out between Alb4 and synthetic capped RNAs as described previously (31, 36) exceptthat the template for RNA transcription was pMH54 or pMH54-S4.The synthetic RNAs contained the entire 3' end of the MHV genomebeginning with the 3' portion of the hemagglutinin esterase geneextending through S, genes 4 and 5, M, and N. For recombination,L2 cells in spinner culture were harvested and infected at a multiplicityof infection of 1 PFU of Alb4 per cell at 33°C. At 2 h postinfection,the cells were washed in phosphate-buffered saline (PBS) withoutcalcium and magnesium and then transfected by electroporationwith the synthetic RNA by using two consecutive pulses from aBio-Rad Gene Pulser apparatus set at 0.3 kV and 960 µF. Infectedand transfected cells were plated onto a monolayer of 17Cl-1 cells,and released virus was harvested at approximately 24 h postinfection.The selection of wild-type recombinants, in which the wild-typeMHV-A59 S gene has been reintroduced, relied on selection againstthe thermolabile, temperature-sensitive, small-plaque phenotypeof Alb4 (14, 31). Briefly, this selection strategy employedheat treatment for 24 h at 40°C in 50 mM Tris-maleate (pH 6.5)-100mM EDTA-10% FBS, plating on L2 monolayers at 39°C, and identificationof viruses exhibiting a large-plaque morphology (compared to theparental Alb4). This strategy was modified to select MHV4 S generecombinants after initial attempts to select recombinant virusesby using heat treatment were unsuccessful. Neutralizing monoclonalantibodies, A2.1 and A2.3, specific for the MHV-A59 S protein(obtained from John O. Fleming, Madison, Wis.) were used to selectagainst viruses that did not express the full-length MHV4 S protein.After recombination, putative recombinant viruses were incubatedfor 1 h at 37°C in the presence of a 1:10 dilution of A2.1 andA2.3 and then plaqued at 39°C on L2 cells. Candidate recombinantswere further analyzed. As described previously, we analyzed forrepair of the Alb4 deletion by detecting size differences in PCRfragments generated from the N gene (31). The recombinant viruseswere then screened for the presence of the 5' portion of the recombinantMHV4 or MHV-A59 S gene. The screen depends on the presence ofthe AvrII site mentioned above. A 988-bp fragment surroundingthe AvrII site was amplified from the genomes of the recombinantviruses, MHV-A59, and Alb4 by using the primers FIJ-79 and RS-221.Digestion of this fragment with AvrII followed by electrophoresisdemonstrated that 19 of 24 MHV4 S gene recombinant viruses containedthe 5' end of the S gene from pMH54-S4. The selected recombinantswere plaque purified once again, and viral stocks were grown on17Cl-1 cells for further analysis (14).

S gene sequencing. For sequencing of the S gene, reverse transcriptase PCR amplification was carried out by cytoplasmic RNA extracted from virus-infectedL2 cells as templates. The oligonucleotides listed in Table 1and described previously (31) were used for amplification ofthe designated regions. Double-stranded PCR products were analyzedby automated sequencing by the Taq dye terminator procedure accordingto the manufacturer's protocol (Taq DyeDeoxy Terminator CycleSequencing Kit; Applied Biosystems). The primers used for amplificationwere also used for sequencing, and each fragment was sequencedin bothdirections.

Viral growth curves. L2 cell monolayers were prepared in 12-well plates in DMEM with 10% FBS. Confluent monolayers were infected with each virus(2 PFU/cell) in duplicate wells and incubated for 1 h at 37°C.After adsorption, the cells were washed with Tris-buffered salinethree times and then fed with 1.5 ml of DMEM-10% FBS. At the timesindicated, the cells were lysed by three cycles of freeze-thawing,and the supernatants were removed and titered by plaque assayon L2 cells as previously described (21).

Inoculation of mice. All animal experiments used 4-week-old MHV-free C57BL/6 mice (The Jackson Laboratory, Bar Harbor, Maine). Mice were anesthetizedwith methoxyflurane (Metofane; Pittman-Moore, Mundelein, Ill.).For intracranial inoculation, the amount of virus designated ineach experiment was diluted in PBS containing 0.75% bovine serumalbumin, and a total volume of 20 µl was injected into the leftcerebral hemisphere. Mock-infected controls were inoculated similarlybut with an uninfected cell lysate at a comparabledilution.

Virulence assays. Fifty-percent lethal dose (LD₅₀) assays were carried out as described previously (23). Mice were inoculated intracraniallywith four- or fivefold serial dilutions of wild-type or recombinantviruses. In two independent experiments, a total of 5 to 15 animalsper dilution per virus were analyzed. Mice were examined for signsof disease or death on a daily basis for up to 21 days postinfection.LD₅₀ values were calculated by the Reed-Muench method (41, 43).

Virus replication in mice. For the measurement of virus replication in the brain and liver, at selected times postinfection, mice were sacrificed andperfused with 10 ml of PBS, and the brains and livers were removed.The left half of each brain was placed directly into 2 ml of isotonicsaline with 0.167% gelatin (gel saline), and the central lobeof the liver was placed in 2 ml of gel saline (39). The righthalf of the brain and a small portion of the liver was used forhistology and viral antigen staining as described below. All organswere weighed and stored frozen at $-$ 80°C until virus titers weredetermined. Organs were homogenized, and virus titers were determinedby plaque assay on L2 cell monolayers (23).

To determine the virus titers after a viral dose of 1 to 2 LD₅₀s (Table 2), mice were inoculated with either 5,000 PFU ofMHV-A59, wtR13, and wtR9 or 10 PFU of MHV4, S4R22, and S4R21,and the virus titers were determined on days 1, 3, 4, 5, and 7postinfection (n = 4). For the kinetic analysis (see Fig. 3),mice were inoculated with 10 PFU of S4R22 or wtR13, and virustiters were determined on days 1, 4, 5, and 7 postinfection (n= 4).

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TABLE 2. Virulence of recombinant viruses and viral titers in the CNS after intracranial inoculation

Histology and immunohistochemistry. For the analysis of inflammation and viral antigen expression, mice were sacrificed at selected times postinfection and perfusedwith 10 ml of PBS, and the brains, spinal cords, and livers wereremoved. The right half of the brain, spinal cord, and a smallportion of the liver were fixed in formalin overnight. (The restof the brain and part of the liver were used for the virus titrationas described above.) Formalin-fixed tissue was embedded in paraffin,sectioned, and left unstained for immunohistochemistry or stainedwith hematoxylin and eosin (H&E) for histologicalanalysis.

Immunohistochemical analysis was performed by the avidin-biotin-immunoperoxidase technique (Vector Laboratories, Burlingame,Calif.) by using diaminobenzadine tetrahydrochloride as a substrate,and a 1:500 dilution of rabbit anti-MHV-A59 serum made againstdetergent-disrupted MHV-A59. Control slides were incubated inparallel with preimmune rabbit serum, and sections from mock-infectedanimals were incubated with rabbit anti-MHV-A59 serum. All slideswere read in a blinded manner. For each of four mice per virus,three sagittal brain sections, separated by 50 µm, were examined,and the number of viral-antigen-positive cells per square millimeterof tissue was determined. For each section, similar regions ofthe brain were studied, and a total of 4 mm² of tissue in the basal forebrain and 2 mm² of tissue in the hippocampus and cingulate gyrus were examined.The number of positively stained cells per square millimeter (seeFig. 6) represents the average number of antigen-positive cellsper square millimeter from all of the sectionsexamined.

H&E-stained histological sections were blinded and independently read by two investigators. The scoring of encephalitis wasbased on a previously described scale (42). One to two sagittalsections from each of four to five mice inoculated with 10 PFUof S4R22 or wtR13 were examined on day 7 postinfection. The intensityof inflammation was scored as follows: 0, normal tissue; 1, mild;2, moderate; and 3, severe. The extent of spread, or the numberof regions involved in inflammation, was scored as follows: 0,normal tissue; 1, mild (less than five regions); 2, moderate (betweensix and seven regions); and 3, severe (more than eight brain regionsinvolved). The specific areas of the brain that were examinedincluded the olfactory bulb, basal forebrain, hippocampus, diencephalon,cingulate gyrus and periventricular areas, neocortex, midbrain,pons, and cerebellum. The final score was the sum of the intensityand extent scores (maximum score of 6). Scores were averaged betweenthe two investigators and presented as the means ± standard deviation.Statistical analysis was done by using the two-sided ttest.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of viruses with recombinant spike genes. In order to study determinants of pathogenesis within the S gene, we used targeted recombination to replace the S gene ofMHV-A59, a mildly neurovirulent strain of MHV, with that of ahighly neurovirulent strain, MHV4 (Fig. 1). Targeted recombinationwas carried out (as described in Materials and Methods) betweensynthetic RNAs transcribed from pMH54-S4 and the recipient virusAlb4, a thermolabile, temperature-sensitive mutant of MHV-A59.The thermolability and temperature-sensitive plaque morphologyof Alb4 is conferred by a deletion in the N gene which may berepaired by recombination with a wild-type N gene; thus, recombinantviruses were initially selected by resistance to heat treatment(14, 31). Attempts to select recombinant viruses containingthe MHV4 S gene by using heat treatment, however, were unsuccessfulsince the MHV4 S gene conferred some degree of thermolabilityto the recombinant viruses (data not shown). Thus, we used a modifiedversion of the selection strategy described previously (14,31). Briefly, neutralizing monoclonal antibodies specific forthe MHV-A59 S protein, A2.1 and A2.3 (11, 20), were used toselect against viruses that expressed the MHV-A59 S protein derivedfrom Alb4 (as described in Materials and Methods). The remainingplaques were therefore enriched for MHV4 S gene recombinants.Because Alb4 is thermolabile and does not replicate efficientlyin animals, it was important to select recombinant viruses withthe wild-type MHV-A59 S and N genes, in the Alb4 background, tobe used as controls instead of Alb4. Wild-type recombinants weregenerated with synthetic RNA transcribed from pMH54, and recombinantviruses were selected by using temperature sensitivity, thermolability,and plaque size as described previously (14, 31).

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FIG. 1. Schematic diagram of targeted recombination and the generated recombinant viruses. The synthetic RNA transcribed from the vector pMH54-S4, encoding the MHV4 S gene, or pMH54, encoding the MHV-A59 S gene, and the corresponding 3' end of the Alb4 genome, derived from MHV-A59, are shown. Viral genes and the sites of the Alb4 deletion are indicated. The curved line between the genome and the synthetic RNA pMH54-S4/pMH54 indicates the region in which a crossover must have occurred. S4R22 and 21 represent the genomes of the MHV4 S gene recombinants, and wtR13 and 9 represent the genomes of the wild-type recombinants. The deletion in the MHV-A59 S gene is indicated. Open bars indicate the MHV-A59 sequence, and closed bars indicate the MHV4 sequence.

The potential recombinants were plaque purified and screened by using PCR amplification and gel electrophoresis for the presenceof the 5' portion of the recombinant S gene and repair of theN gene deletion (14, 31). This screen was facilitated by theintroduction of an AvrII restriction site in the signal sequenceof the recombinant S gene (as described in Materials and Methods).For both the MHV4 S gene-containing and MHV-A59 S gene-containingrecombinants, we characterized two independently derived recombinantsisolated from separate recombination events. The MHV4 S gene recombinantswere named S4R22 and S4R21, and the wild-type recombinants werenamed wtR13 andwtR9.

To verify that no secondary site mutations had been introduced into the S gene, we sequenced the 3' portion of the hemagglutininesterase open reading frame through to the 3' end of the S gene.The sequencing of the S genes of the four recombinant virusesrevealed that only one silent mutation (C to T) had been introducedat nucleotide 2159 of S4R21. The sequence of the S gene from theMHV4 S gene recombinants and the cloning plasmid used to generatethem, pSwt, was identical to the previously published sequenceof the MHV4 S gene (37) except for a previously noted silentmutation at nucleotide 3990 (18) and a three-nucleotide mutation(CTG in published sequence to GCT in cloned DNA), which resultedin an amino acid change at position 255 (leucine to alanine).Recombinant viruses that contained the two restriction sites,AvrII and SbfI, and were repaired in the N gene were likely theresult of single recombination events 5' to the S gene. Threeof the four recombinant viruses contained all three markers, butanalysis of wtR9 revealed that it contained the AvrII restrictionsite and the repaired N gene but not the 3' SbfI restriction site.Thus, wtR9 underwent at least three recombination events, oneof which was within the S gene. Since the sequence of the S geneof Alb4 is identical to that of MHV-A59, we were not able to determinethe exact location of the recombination event withinS.

In vitro growth characteristics of the recombinant viruses. In cell culture, MHV4 and MHV-A59 show very different replication properties. While MHV-A59 replicates to a high titer ina number of cell lines, it has been shown that MHV4 replicatesto a lower titer and displays higher levels of fusion and cytotoxicity(5, 19, 40). To determine whether the recombinant viruses,differing in S, exhibited altered replication in L2 cells, wecompared their replication to that of MHV4 and MHV-A59. Single-stepgrowth curves were performed, and the results (Fig. 2) indicatethat the pattern of replication segregated with the S gene. Therecombinant viruses containing the MHV4 S gene (S4R22 and S4R21)and wild-type MHV4 demonstrated a decrease in the extent of viralreplication compared to viruses containing the MHV-A59 S gene,wtR13, wtR9, and MHV-A59. In addition, the S gene also determinedthe plaque morphology. At 48 h after the infection of L2 monolayers,MHV-A59 and the wild-type recombinants exhibited a large-plaquephenotype (>2 mm), while MHV4 and the MHV4 S gene recombinantsexhibited a small-plaque phenotype (<1 mm) (data not shown). Thus,in cell culture the S gene of MHV4 conferred an alteration inviral replication and plaque morphology.

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FIG. 2. Time course of recombinant virus production in L2 cell cultures. L2 cells were infected in duplicate with MHV-A59 ( $open circle$ ), wtR13 (

), wtR9 (

), MHV4 (

), S4R22 ( $black-triangle$ ), and S4R21 ( $triangle$ ) at a multiplicity of infection of 2 PFU/cell. At the indicated times, cells and cell culture supernatant were freeze-thawed three times and clarified, and virus titers were then determined by plaque assay. Each point represents the mean titer of duplicate samples.

Virulence of recombinant viruses. Using isogenic recombinant viruses that differ exclusively in the S gene, we sought to determine whether the S gene of thehighly neurovirulent MHV4 virus was sufficient to alter the virulenceof the recombinant viruses. Thus, mice were inoculated intracraniallywith serial dilutions of S4R22 and S4R21, containing the MHV4spike, wtR13 and wtR9, containing the MHV-A59 spike, wild-typeMHV4, and wild-type MHV-A59. Infected mice were observed for lethalityand an LD₅₀ was calculated for each virus. The results are shownin Table 2. The recombinant viruses containing the MHV4 S gene(S4R22 and S4R21) displayed a dramatically lower LD₅₀ value ora more virulent phenotype than the wild-type recombinants (wtR13and wtR9). As expected, wtR13 and wtR9 displayed an LD₅₀ similarto that of MHV-A59. The LD₅₀ value for wild-type MHV4 was similarto that of the MHV4 S gene recombinants. Thus, the MHV4 S genewas able to confer a significantly more virulentphenotype.

Clinical signs also segregated with the spike gene. Mice inoculated with approximately 1 to 2 LD₅₀s, 5,000 PFU, of the MHV-A59spike-containing viruses (wtR13, wtR9, or MHV-A59) exhibited delayedweight gain and growth early in infection (data not shown). Miceinoculated with approximately 1 to 2 LD₅₀s, 10 PFU, of the MHV4spike-containing viruses (S4R22, S4R21, or MHV4) appeared normalup until days 4 to 6 postinfection, when all mice began to exhibitclinical signs such as hunched posture, ruffled fur, and abnormalgait (data notshown).

Recombinant virus replication in the brains and livers of infected mice. The recombinants containing the MHV4 S gene (S4R22 and S4R21) were dramatically more virulent than the recombinants containingthe MHV-A59 S gene (wtR13 and wtR9). To determine whether thelocation or extent of viral replication was altered for the recombinantviruses, we infected animals intracranially with virus and determinedthe titers of the virus in the brains and livers at various timespostinfection as described in Materials andMethods.

Initially, we compared the viral replication in the brain of S4R22, S4R21, MHV4, wtR13, wtR9, and MHV-A59 by using approximately1 to 2 times the LD₅₀ for each virus. Infection at this dose allowedus to compare the replication patterns of each virus at a dosewhich resulted in roughly equal mortality. Mice were inoculatedintracranially with 10 PFU of the MHV4 spike-containing viruses(S4R22, S4R21, and MHV4) and 5,000 PFU of the MHV-A59 spike-containingviruses (wtR9, wtR13, and MHV-A59). The peak viral titers areshown in Table 2. As expected, the kinetics and final extentof replication in the brain of wtR13, wtR9, and MHV-A59 were similar.Infection with only 10 PFU of MHV4 also resulted in a similarfinal extent of viral replication. Despite having a similar virulence,the MHV4 S gene recombinants, S4R22 and S4R21, exhibited significantlylower levels of viral replication than wild-typeMHV4.

To compare the abilities of the MHV4 spike- and MHV-A59 spike-containing viruses to replicate in the brain and liver, we infectedanimals intracranially with 10 PFU of either S4R21, S4R22, wtR13,or wild-type MHV4. At this dose, more than half of the mice infectedwith a MHV4 S gene-containing virus would be expected to die,whereas none of the mice infected with wtR13 would be expectedto die. The viral titers in the brains and livers were determinedat various times postinfection (Fig. 3). In the brain, the MHV4spike- and MHV-A59 spike-containing recombinant viruses exhibitednearly identical replication both in terms of the extent of replicationand the kinetics. The wild-type MHV4 virus, which shares onlythe spike gene with the MHV4 S gene recombinants, replicated toa higher titer than did the recombinant viruses. At this dose,viral replication in the liver was at or below the limit of detection(500 PFU/g), and histologic examination of the livers revealedlittle to no hepatitis (data not shown) for both the MHV4 S geneand wild-type recombinants. Thus, despite the striking differencein virulence after inoculation with 10 PFU of virus, the MHV4S gene recombinants and the wild-type recombinants showed similarlevels of viral replication in the brain and minimal replicationin the liver.

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FIG. 3. Viral replication in the brains and livers of animals after intracranial inoculation. C57BL/6 weanling mice were infected with 10 PFU of MHV4 (

), S4R22 ( $black-triangle$ ), S4R21 ( $triangle$ ), and wtR13 (

). Animals were sacrificed at the indicated times, and virus titers in the brains (A) or livers (B) were determined by plaque assay. The limit of detection was 500 PFU/g of tissue. The data shown represent the means (and standard deviations) of the titers from eight (S4R22) or four (all other viruses) animals.

Distribution of viral antigen in the brains of infected animals. To examine the possibility that the MHV4 S gene recombinants had an altered pattern of viral spread within the brain, we usedimmunohistochemistry to determine the distribution of viral antigen.Brain sections from animals infected with 10 PFU of S4R22, S4R21,wtR13, or wild-type MHV4 at day 3 or 4, day 5, and day 7 postinfectionwere stained with polyclonal antisera against MHV proteins, blinded,and examined. At the peak of viral antigen expression, on day5 postinfection, brain sections from a total of four animals pervirus were examined and representative sections are shown in Fig.4. The MHV4 S gene-containing viruses, S4R22, S4R21, and wild-typeMHV4 exhibited similar patterns of antigen staining which differedin two ways from those seen after infection with the MHV-A59 spike-containingvirus, wtR13. In some areas of the brain, such as the basal forebrain(Fig. 4A and 4B), the number of antigen-positive cells per regionwas greater for the MHV4 S gene recombinants than for the wild-typerecombinant, wtR13. In other regions of the brain, such as thehippocampus (Fig. 4C and D), the MHV4 S gene recombinants exhibitedpositive antigen staining, whereas similar brain regions fromwtR13-infected animals were negative for viral antigen staining.To quantify the differences in the intensity and extent of positiveantigen staining that were observed between the MHV4 S gene- andthe MHV-A59 S gene-containing viruses, the number of antigen-positivecells per square millimeter of brain tissue was determined inthe basal forebrain, cingulate gyrus, and hippocampus (Fig. 5).These three regions were selected since they reflected the rangeof differences which were seen between the two recombinant viruses.In the cingulate gyrus and the hippocampus, the number of antigen-positivecells was significantly greater for the animals infected withthe MHV4 S gene recombinant, S4R22, than for the animals infectedwith the wild-type recombinant, wtR13 (two-tailed t test; P <0.001 and P < 0.01, respectively). In the basal forebrain therewas less disparity between the two recombinant viruses, yet thedifference was still statistically significant (two-tailed t test,P < 0.05). As determined by morphology, the MHV4 S gene- and MHV-A59S gene-containing viruses, including both wild-type and recombinantviruses, exhibited positive antigen staining of neuronal and nonneuronalcell types with no obvious differences in cell type.

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FIG. 4. Immunohistochemistry of the brains of C57BL/6 mice infected with recombinant viruses. Mice were infected as described for Fig. 3 and then sacrificed at 5 days postinfection. Brains were removed, fixed, and sectioned, and MHV proteins were detected by immunolabeling with rabbit anti-MHV-A59 serum. (A) S4R22-infected brain shows severe viral antigen staining in the basal forebrain. (B) wtR13-infected brain shows moderate viral antigen staining in the basal forebrain. In both panels A and B antigen staining is evident in the cytoplasm of neurons. High-power magnification of the hippocampus demonstrates viral antigen staining of a neuron in S4R22-infected brain (C) and the absence of antigen staining in wtR13-infected brain (D). Magnification: A and B, ×190; C and D, ×380.

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FIG. 5. Viral-antigen-positive cells in the hippocampus, cingulate gyrus, and basal forebrain of mice infected with recombinant viruses. Mice were infected as for Fig. 3 and sacrificed at 5 days postinfection. Brains were removed, fixed, and sectioned, and MHV proteins were detected by immunolabeling with rabbit anti-MHV-A59 serum. All sections were blinded, and the numbers of viral-antigen-positive cells per square millimeter of tissue in the basal forebrain (BF), cingulate gyrus (CG), and hippocampus (Hippo) were determined by averaging the number of positive cells per square millimeter in three sagittal sections from each of four animals per virus. Error bars indicate the standard error of the mean. The S4R22 virus-infected mice (closed bars) exhibited significantly more antigen-positive cells than did the wtR13 virus-infected mice (open bars). *, P < 0.05; **, P < 0.01; ***, P < 0.001 (two-sided t test).

Distribution and extent of histopathology in the brains of infected animals. The results of immunohistochemical examination suggested that infection with the MHV4 spike-containing recombinants resultedin a more intense and extensive infection of the CNS comparedto infection with the MHV-A59 spike-containing recombinants. Todetermine whether the inflammatory response to infection withthe MHV4 spike-containing recombinants was altered, we examinedthe severity of encephalitis induced by the recombinant viruses.Brain and spinal cord sections from infected mice were obtainedon days 3 or 4, day 5, and day 7 postinfection, and stained withH&E to assess the severity ofinflammation.

At the peak of inflammation 7 days postinfection with 10 PFU of virus, the MHV4 spike-containing viruses (S4R22, S4R21, andMHV4) caused a more intense and extensive inflammatory responsethan did the MHV-A59 spike-containing virus, wtR13. Representativesections from a total of four (MHV4 and S4R21), five (wtR13),or eight (S4R22) infected animals (Fig. 6) illustrate that theMHV4 S gene-containing viruses induced a dramatic degree of perivascularcuffing and inflammation (Fig. 6A and C), while infection withwtR13 resulted in less severe inflammation (Fig. 6B and D). Theoverall distribution of inflammation was as described in previousreports for MHV4, another JHM strain (MHV-JHM), and MHV-A59 (2,13, 28, 30). The regions most consistently involved includedthe olfactory system, the piriform and entorhinal cortices, basalforebrain structures such as the septal nuclei and piriform cortices,the amygdala complex, regions of the diencephalon and basal ganglia,the periventricular areas and cingulate gyrus, regions of thehippocampus, the neocortex, and the brain stem.

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FIG. 6. Histopathology of the brains of C57BL/6 mice infected with recombinant viruses. Mice were infected intracranially as for Fig. 3 and sacrificed at 7 days postinfection. Brains were removed, fixed, sectioned, and stained with H&E as described in Materials and Methods. (A) S4R22-infected brain shows multiple large foci of inflammation in the midbrain and pons. (B) wtR13-infected brain shows a few small foci of inflammation in the midbrain and pons. (C) Higher magnification of the S4R22-infected brain shown in panel A demonstrates severe perivascular cuffing. (D) Higher magnification of the wtR13-infected brain shown in panel B shows moderate perivascular cuffing. Magnification: A and B, ×190; C and D, ×380.

In order to provide a more quantitative interpretation of these data, histologic sections from mice infected with 10 PFU ofS4R22, containing the MHV4 spike, or wtR13, containing the MHV-A59spike, were blinded and scored by two independent reviewers (asdescribed in Materials and Methods). The histologic score, representingboth the intensity of inflammation and the extent, or the numberof brain regions exhibiting inflammation, was significantly greaterfor S4R22 (4.8 ± 0.6) compared to wtR13 (3.5 ± 0.9) (two-tailedt test; P < 0.001).

To determine whether infection with a high dose of the MHV-A59 spike-containing viruses could reproduce the intense inflammationseen with 10 PFU of the MHV4 spike-containing viruses, mice wereinfected with a dose of 1 to 2 LD₅₀s, 5,000 PFU, of the MHV-A59spike-containing viruses (wtR13, wtR9, and MHV-A59). Once again,the intensity and extent of inflammation was decreased relativeto that induced by the MHV4 spike-containing viruses, yet thelocation of inflammation was similar (data not shown). The peakof inflammation was slightly earlier at this dose (day 5 or 7postinfection). Thus, the intensity of inflammation seen witha dose of approximately 1 to 2 LD₅₀s is greater for the MHV4 Sgene recombinants than for the MHV-A59 S gene recombinants. Overall,these data demonstrate that the MHV4 spike-containing virusesexhibited an increase in the intensity and the extent of inflammationrelative to the MHV-A59 spike-containingviruses.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Previous studies have suggested a correlation between mutations in S and alterations in virulence; however, these studieshave been limited by the lack of technology to isolate mutationsin the same genetic background. The use of targeted recombinationhas allowed us to begin to definitively map specific phenotypicproperties to the S protein. In our recent study (31), a specificmutation in the S gene, introduced by targeted recombination,was found to alter the pathogenesis of the virus. We have usedthe targeted recombination technique here to directly addressthe role of the MHV4 S gene in pathogenesis and virulence. Bycomparing recombinant viruses, which differ exclusively in theS gene, we have been able to characterize the effect of S onneurovirulence.

For each desired recombinant virus, we studied at least two independently isolated recombinants to ensure that spurious mutationsintroduced during viral replication did not interfere with ourinterpretations. In cell culture and in vivo, the two MHV4 S generecombinant viruses, S4R22 and S4R21, exhibited identical phenotypicproperties. The wild-type recombinants also demonstrated phenotypicproperties similar to each other and to MHV-A59. Due to the similarityin pathogenic properties within each group of recombinant virusesand the striking differences between MHV-A59 and MHV4 spike-containingviruses, we attributed differences in pathogenesis between theMHV4 S gene recombinants and the wild-type recombinants to alterationsin the Sgene.

One of the wild-type recombinants, wtR9, showed a slightly lower LD₅₀ than did MHV-A59. This is most likely the result ofa mutation(s) outside of S, acquired during recombination or subsequentviral passage. To verify that wtR9 was an exception and that wtR13was a representative wild-type recombinant, we determined theLD₅₀ of an additional wild-type recombinant, wtR2, and found itto be similar to both wtR13 and MHV-A59, with a log₁₀(LD₅₀) of3.4. In addition, a previously characterized wild-type recombinant,wtR10, displayed virulence identical to that of MHV-A59 (31).

After intracranial inoculation, the pathogenesis of the recombinant viruses containing the MHV4 S gene was clearly differentfrom that of the recombinants containing the MHV-A59 S gene. Asmeasured by LD₅₀, the MHV4 S gene conferred a dramatic increasein virulence, and this virulence was associated with increasedviral antigen expression and inflammation in the CNS and viralreplication in the brain but not in the liver. Comparison of theviral replication in the brain of the MHV4 spike- and MHV-A59spike-containing viruses, however, revealed that they replicatedwith similar kinetics and to a similar final extent (Fig. 3).Thus, the neurovirulence of the MHV4 S gene-containing recombinantsrelative to the MHV-A59 S gene-containing recombinants could notbe attributed to a higher load of infectious virus in the brain.In support of this observation that neurovirulence is not correlatedwith replication levels, peak viral titers for wild-type MHV4and the MHV4 S gene recombinants were nearly 100-fold differentdespite a similar virulence. This variation in viral replicationbetween the recombinant viruses and wild-type MHV4 must be attributableto genetic differences outside of the Sgene.

There are several possible mechanisms by which the MHV4 spike may confer an increase in neurovirulence. To begin it is helpfulto compare the primary structure of the S glycoprotein of MHV4(37) and MHV-A59 (35). Within S2 the amino acid sequence identityis quite high, 96%, but in S1 there is more variation, with lessthan 89% identity. In addition, a single amino acid differencein the cleavage site of MHV-A59 relative to MHV4 has been shownto decrease the efficiency of cleavage of the S protein (6).The most striking difference between the two S genes, however,is a large deletion of 52 amino acids in the HVR of MHV-A59 (37).

One possible explanation for the difference in neurovirulence between the MHV4 S gene recombinants and the MHV-A59 S generecombinants is that the MHV4 S protein is more cytotoxic. Anincrease in viral cytotoxicity, particularly of nonrenewable cellssuch as neurons, could dramatically affect host survival. Fromthe study of neuroattenuated mutant viruses an association hasbeen made between deletions in the HVR and diminished cytopathiceffects in tissue culture (19). Furthermore, it has been suggestedthat the fusion potential of the spike is related to its abilityto induce cytotoxicity and that this cytotoxicity may be due inpart to intracellular fusion (40). Thus, the more fusogenicMHV4 spike would induce more cytotoxicity than the less fusogenicMHV-A59 spike. An additional mechanism of cell death, virus-inducedapoptosis, has been associated with neurovirulence in Sindbisvirus (32). Although the role of apoptosis in MHV neurovirulenceis not known, MHV-induced apoptosis has been reported in macrophages(3).

A second possible mechanism to explain the neurovirulence conferred by the MHV4 S gene is related to the rate or extent ofthe spread of the virus and stems from the study of a neuroattenuatedmutant of MHV4, V5A13.1, which was selected for resistance toneutralizing monoclonal antibodies (10). Characterization ofthis variant virus in vivo revealed that, relative to MHV4, ithad a decreased rate of spread and decreased viral replicationin the brain (13). Although the mechanism of decreased spreadis not known, it is speculated that decreased fusogenicity mayplay a role (19). The MHV4 S gene recombinants exhibited a greateramount of viral antigen expression than did the MHV-A59 S generecombinants. However, we did not detect a difference in the extentof viral replication in the brain. One possible explanation isthat the MHV4 S gene-containing recombinants spread more quicklyfrom cell to cell yet produced less infectious virus per cellthan did the MHV-A59 spike-containingviruses.

The outcome of viral infection is determined by the complex interaction between the virus and the host immune system. Thus,a study of MHV pathogenesis must take into consideration the immuneresponse to the virus. The S protein is a target of both neutralizingand cell-mediated immunity, and studies with the JHM strain ofMHV have identified two CD8⁺ T-cell epitopes in the S glycoprotein (4, 7). Interestingly,the more immunodominant epitope, encompassing amino acids 510to 518, within the HVR of S1, is deleted in MHV-A59. Thus, itis possible that the immune response to this epitope contributesto the intense inflammation and overall neurovirulence of theMHV4 S gene. Alternatively, the MHV4 S protein may stimulate analtered immune response that is ultimately more neurotoxic. Ashas been shown with a number of viruses, including MHV and Sindbisvirus, the stimulation of specific immune modulators can mediatedisease severity (27, 33, 38). Thus, either global immunestimulation or stimulation of specific immune mediators may playa role in determining the neurovirulence of various Sproteins.

We have shown, by using targeted homologous recombination, that the MHV4 S gene contains determinants of neurovirulence. Thisfinding demonstrates unambiguously what has been suggested byearlier studies associating mutations in S with alterations inneurovirulence. Future studies will be directed at precisely definingwhich functional regions of the MHV4 S gene are necessary andsufficient to confer this neurovirulent phenotype. In addition,we will investigate the immune response to the recombinant viruses.With this knowledge we hope to gain a better understanding ofthe mechanism of MHV-induced neurologicdisease.

	ACKNOWLEDGMENTS

This work was supported by Public Health Service grants NS-30606 and NS-21954 (S.R.W.) and a National Multiple Sclerosis Societygrant RG-2615A1/2 (E.L.). J.J.P. was supported in part by traininggrant GM-07229.

We thank Paul Masters for pMH54, Alb4, and advice throughout the project; Michael J. Buchmeier for pSwt and MHV4; and JohnO. Fleming for monoclonal antibodies A2.1 and A2.3. We thank JeanTsai for kindly providing wtR13, Su-hun Seo for excellent technicalassistance, and Luis M. Schang, Jean Tsai, and Henry Teng forcritical reading of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, University of Pennsylvania, 203A Johnson Pavilion, 36thSt. and Hamilton Walk, Philadelphia, PA 19104-6076. Phone: (215)898-8013. Fax: (215) 573-4858. E-mail: weisssr{at}mail.med.upenn.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bailey, O. T., A. M. Pappenheimer, F. S. Cheever, and J. B. Daniels. 1949. A murine virus (JHM) causing disseminated encephalomyelitis with extensive destruction of myelin. II. Pathology. J. Exp. Med. 90:195-212[Abstract].

2. Barnett, E. M., M. D. Cassell, and S. Perlman. 1993. Two neurotropic viruses, herpes simplex virus type 1 and mouse hepatitis virus, spread along different neural pathways from the main olfactory bulb. Neuroscience 57:1007-1025[Medline].

3. Belyavskyi, M., E. Belyavskaya, G. A. Levy, and J. L. Leibowitz. 1998. Coronavirus MHV-3-induced apoptosis in macrophages. Virology 250:41-49[Medline].

4. Bergmann, C. C., Q. Yao, M. Lin, and S. A. Stohlman. 1996. The JHM strain of mouse hepatitis virus induces a spike protein-specific Db-restricted cytotoxic T cell response. J. Gen. Virol. 77:315-325[Abstract/Free Full Text].

5. Bond, C. W., J. L. Leibowitz, and J. A. Robb. 1979. Pathogenic murine coronaviruses: II. Characterization of virus-specific proteins of murine coronaviruses JHMV and A59V. Virology 94:371-384[Medline].

6. Bos, E. C. W., L. Heijnen, W. Luytjes, and W. J. M. Spaan. 1995. Mutational analysis of the murine coronavirus spike protein: effect on cell-to-cell fusion. Virology 214:453-463[Medline].

7. Castro, R. F., and S. Perlman. 1995. CD8⁺ T-cell epitopes within the surface glycoprotein of a neurotropic coronavirus and correlation with pathogenicity. J. Virol. 69:8127-8131[Abstract].

8. Collins, A. R., R. L. Knobler, H. Powell, and M. J. Buchmeier. 1982. Monoclonal antibodies to murine hepatitis virus-4 (strain JHM) define the viral glycoprotein responsible for attachment and cell-cell fusion. Virology 119:358-371[Medline].

9. Compton, S. R., S. W. Barthold, and A. L. Smith. 1993. The cellular and molecular pathogenesis of coronaviruses. Lab. Anim. Sci. 43:15-28[Medline]. [Erratum 43:203.]

10. Dalziel, R. G., P. W. Lampert, P. J. Talbot, and M. J. Buchmeier. 1986. Site-specific alteration of murine hepatitis virus type 4 peplomer glycoprotein E2 results in reduced neurovirulence. J. Virol. 59:463-471[Abstract/Free Full Text].

11. Daniel, C., R. Anderson, M. J. Buchmeier, J. O. Fleming, W. J. M. Spaan, H. Wege, and P. J. Talbot. 1993. Identification of an immunodominant linear neutralization domain on the S2 portion of the murine coronavirus spike glycoprotein and evidence that it forms part of complex tridimensional structure. J. Virol. 67:1185-1194[Abstract/Free Full Text].

12. DeGroot, R. J., W. Luytjes, M. C. Horzinek, B. A. M. van der Zeijst, W. J. M. Spaan, and J. A. Lenstra. 1987. Evidence for a coiled-coil structure in the spike proteins of coronaviruses. J. Mol. Biol. 196:963-966[Medline].

13. Fazakerley, J. K., S. E. Parker, F. Bloom, and M. J. Buchmeier. 1992. The V5A13.1 envelope glycoprotein deletion mutant of mouse hepatitis virus type-4 is neuroattenuated by its reduced rate of spread in the central nervous system. Virology 187:178-188[Medline].

14. Fischer, F., C. F. Stegen, C. A. Koetzner, and P. S. Masters. 1997. Analysis of a recombinant mouse hepatitis virus expressing a foreign gene reveals a novel aspect of coronavirus transcription. J. Virol. 71:5148-5160[Abstract].

15. Fleming, J. O., M. D. Trousdale, F. A. K. El-Zaatari, S. A. Stohlman, and L. P. Weiner. 1986. Pathogenicity of antigenic variants of murine coronavirus JHM seleced with monoclonal antibodies. J. Virol. 58:869-875[Abstract/Free Full Text].

16. Frana, M. F., J. N. Behnke, L. S. Sturman, and K. V. Holmes. 1985. Proteolytic cleavage of the E2 glycoprotein of murine coronavirus: host-dependent differences in proteolytic cleavage and cell fusion. J. Virol. 56:912-920[Abstract/Free Full Text].

17. Gallagher, T. M. 1997. A role for naturally occurring variation of the murine coronavirus spike protein in stabilizing association with the cellular receptor. J. Virol. 71:3129-3137[Abstract].

18. Gallagher, T. M., C. Escarmis, and M. J. Buchmeier. 1991. Alteration of pH dependence of coronavirus-induced cell fusion: effect of mutations in the spike glycoprotein. J. Virol. 65:1916-1928[Abstract/Free Full Text].

19. Gallagher, T. M., S. E. Parker, and M. J. Buchmeier. 1990. Neutralization-resistant variants of a neurotropic coronavirus are generated by deletions within the amino-terminal half of the spike glycoprotein. J. Virol. 64:731-741[Abstract/Free Full Text].

20. Gilmore, W., J. O. Fleming, S. A. Stohlman, and L. P. Weiner. 1987. Characterization of the structural proteins of the murine coronavirus strain A59 using monoclonal antibodies. Proc. Soc. Exp. Biol. Med. 185:177-186[Medline].

21. Gombold, J. L., S. T. Hingley, and S. R. Weiss. 1993. Fusion-defective mutants of mouse hepatitis virus A59 contain a mutation in the spike protein cleavage signal. J. Virol. 67:4504-4512[Abstract/Free Full Text].

22. Higuchi, R. 1990. PCR protocols: a guide to methods and applications, p. 177-183. Academic Press, Inc., San Diego, Calif.

23. Hingley, S. T., J. L. Gombold, E. Lavi, and S. R. Weiss. 1994. MHV-A59 fusion mutants are attenuated and display altered hepatotropism. Virology 200:1-10[Medline].

24. Houtman, J. J., and J. O. Fleming. 1996. Pathogenesis of mouse hepatitis virus-induced demyelination. J. Neurovirol. 2:361-376[Medline].

25. Koetzner, C. A., M. M. Parker, C. S. Ricard, L. S. Sturman, and P. S. Masters. 1992. Repair and mutagenesis of the genome of a deletion mutant of the murine coronavirus mouse hepatitis virus by targeted RNA recombination. J. Virol. 66:1841-1848[Abstract/Free Full Text].

26. Kubo, H., Y. K. Yamada, and F. Taguchi. 1994. Localization of neutralizing epitopes and the receptor-binding site within the amino-terminal 330 amino acids of the murine coronavirus spike protein. J. Virol. 68:5403-5410[Abstract/Free Full Text].

26a. Kuo, L., G.-J. Godeke, M. J. B. Raamsman, P. S. Masters, and P. J. M. Rottier. Retargeting of coronavirus by substitution of the spike glycoprotein ectodomain: crossing the host species barrier. Submitted for publication.

27. Lane, T. E., H. S. Fox, and M. J. Buchmeier. 1999. Inhibition of nitric oxide synthase-2 reduces the severity of mouse hepatitis virus-induced demyelination: implications for NOS2/NO regulation of chemokine expression and inflammation. J. Neurovirol. 5:48-54[Medline].

28. Lavi, E., P. S. Fishman, M. K. Highkin, and S. R. Weiss. 1988. Limbic encephalitis after inhalation of a murine coronavirus. Lab. Invest. 58:31-36[Medline].

29. Lavi, E., D. H. Gilden, M. K. Highkin, and S. R. Weiss. 1986. The organ tropism of mouse hepatitis virus strain A59 is dependent on dose and route of inoculation. Lab. Anim. Sci. 36:130-135[Medline].

30. Lavi, E., E. M. Murray, S. Makino, S. A. Stohlman, M. M. C. Lai, and S. R. Weiss. 1990. Determinants of coronavirus MHV pathogenesis are localized to 3' portions of the genome as determined by ribonucleic acid-ribonucleic acid recombination. Lab. Invest. 62:570-578[Medline].

31. Leparc-Goffart, I., S. T. Hingley, M. M. Chua, J. Phillips, E. Lavi, and S. R. Weiss. 1998. Targeted recombination within the spike gene of murine coronavirus mouse hepatitis virus-A59: Q159 is a determinant of hepatotropism. J. Virol. 72:9628-9636[Abstract/Free Full Text].

32. Lewis, J., S. L. Wesselingh, D. E. Griffin, and J. M. Hardwick. 1996. Alphavirus-induced apoptosis in mouse brains correlates with neurovirulence. J. Virol. 70:1828-1835[Abstract].

33. Liang, X. H., J. E. Goldman, H. H. Jiang, and B. Levine. 1999. Resistance of interleukin-1B-deficient mice to fatal Sindbis encephalitis. J. Virol. 73:2563-2567[Abstract/Free Full Text].

34. Luo, Z., and S. R. Weiss. 1998. Roles in cell-to-cell fusion of two conserved hydrophobic regions in the murine coronavirus spike protein. Virology 244:483-494[Medline].

35. Luytjes, W., L. S. Sturman, P. J. Bredenbeck, J. Charite, B. A. M. van der Zeijst, M. C. Horzinek, and W. J. M. Spaan. 1987. Primary structure of the glycoprotein E2 of coronavirus MHV-A59 and identification of the trypsin cleavage site. Virology 161:479-487[Medline].

36. Masters, P. S., C. A. Koetzner, C. A. Kerr, and Y. Heo. 1994. Optimization of targeted RNA recombination and mapping of a novel nucleocapsid gene mutation in the coronavirus mouse hepatitis virus. J. Virol. 68:328-337[Abstract/Free Full Text].

37. Parker, S. E., T. M. Gallagher, and M. J. Buchmeier. 1989. Sequence analysis reveals extensive polymorphism and evidence of deletions within the E2 glycoprotein gene of several strains of murine hepatitis virus. Virology 173:664-673[Medline].

38. Pope, M., P. A. Marsden, E. Cole, S. Sloan, L. S. Fung, Q. Ning, J. W. Ding, J. L. Leibowitz, M. J. Phillips, and G. A. Levy. 1998. Resistance to murine hepatitis virus strain 3 is dependent on production of nitric oxide. J. Virol. 72:7084-7090[Abstract/Free Full Text].

39. Ramig, R. F. 1982. Isolation and genetic characterization of temperature sensitive mutants of simian rotavirus SA11. Virology 120:93-135[Medline].

40. Rao, P. V., and T. M. Gallagher. 1998. Intracellular complexes of viral spike and cellular receptor accumulate during cytopathic murine coronavirus infections. J. Virol. 72:3278-3288[Abstract/Free Full Text].

41. Reed, L. J., and H. Muench. 1938. A simple method of estimating fifty per cent points. Am. J. Hyg. 27:493-497.

42. Sasseville, V. G., M. M. Smith, C. R. Mackay, D. R. Pauley, K. G. Mansfield, D. J. Ringler, and A. A. Lackner. 1996. Chemokine expression in simian immunodeficiency virus-induced AIDS encephalitis. Am. J. Pathol. 149:1459-1467[Abstract].

43. Smith, A. L., and S. W. Barthold. 1997. Methods in viral pathogenesis, p. 483-506. In N. Nathanson (ed.), Viral pathogenesis. Lippincott-Raven, Philadelphia, Pa.

44. Sturman, L. S., C. S. Ricard, and K. V. Holmes. 1985. Proteolytic cleavage of the E2 glycoprotein of murine coronavirus: activation of cell fusing activity of virions by trypsin and separation of two different 90K cleavage fragments. J. Virol. 56:904-911[Abstract/Free Full Text].

45. Wege, H., J. Winter, and R. Meyermann. 1988. The peplomer protein E2 of coronavirus JHM as a determinant of neurovirulence: definition of critical epitopes by variant analysis. J. Gen. Virol. 69:87-98[Abstract/Free Full Text].

46. Williams, R. K., G. S. Jiang, and K. V. Holmes. 1991. Receptor for mouse hepatitis virus is a member of the carcinoembryonic antigen family of glycoproteins. Proc. Natl. Acad. Sci. USA 88:5533-5536[Abstract/Free Full Text].

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Thorp, E. B., Boscarino, J. A., Logan, H. L., Goletz, J. T., Gallagher, T. M. (2006). Palmitoylations on Murine Coronavirus Spike Proteins Are Essential for Virion Assembly and Infectivity. J. Virol. 80: 1280-1289 [Abstract] [Full Text]
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Tsai, J. C., Zelus, B. D., Holmes, K. V., Weiss, S. R. (2002). The N-Terminal Domain of the Murine Coronavirus Spike Glycoprotein Determines the CEACAM1 Receptor Specificity of the Virus Strain. J. Virol. 77: 841-850 [Abstract] [Full Text]
Lewicki, D. N., Gallagher, T. M. (2002). Quaternary Structure of Coronavirus Spikes in Complex with Carcinoembryonic Antigen-related Cell Adhesion Molecule Cellular Receptors. J. Biol. Chem. 277: 19727-19734 [Abstract] [Full Text]
Kuo, L., Masters, P. S. (2002). Genetic Evidence for a Structural Interaction between the Carboxy Termini of the Membrane and Nucleocapsid Proteins of Mouse Hepatitis Virus. J. Virol. 76: 4987-4999 [Abstract] [Full Text]
Navas, S., Seo, S.-H., Chua, M. M., Sarma, J. D., Lavi, E., Hingley, S. T., Weiss, S. R. (2001). Murine Coronavirus Spike Protein Determines the Ability of the Virus To Replicate in the Liver and Cause Hepatitis. J. Virol. 75: 2452-2457 [Abstract] [Full Text]
Evans, S., Cavanagh, D., Britton, P. (2000). Utilizing fowlpox virus recombinants to generate defective RNAs of the coronavirus infectious bronchitis virus. J. Gen. Virol. 81: 2855-2865 [Abstract] [Full Text]
Das Sarma, J., Fu, L., Tsai, J. C., Weiss, S. R., Lavi, E. (2000). Demyelination Determinants Map to the Spike Glycoprotein Gene of Coronavirus Mouse Hepatitis Virus. J. Virol. 74: 9206-9213 [Abstract] [Full Text]
Hsue, B., Hartshorne, T., Masters, P. S. (2000). Characterization of an Essential RNA Secondary Structure in the 3' Untranslated Region of the Murine Coronavirus Genome. J. Virol. 74: 6911-6921 [Abstract] [Full Text]
Kuo, L., Godeke, G.-J., Raamsman, M. J. B., Masters, P. S., Rottier, P. J. M. (2000). Retargeting of Coronavirus by Substitution of the Spike Glycoprotein Ectodomain: Crossing the Host Cell Species Barrier. J. Virol. 74: 1393-1406 [Abstract] [Full Text]

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1.	Bailey, O. T., A. M. Pappenheimer, F. S. Cheever, and J. B. Daniels. 1949. A murine virus (JHM) causing disseminated encephalomyelitis with extensive destruction of myelin. II. Pathology. J. Exp. Med. 90:195-212[Abstract].
2.	Barnett, E. M., M. D. Cassell, and S. Perlman. 1993. Two neurotropic viruses, herpes simplex virus type 1 and mouse hepatitis virus, spread along different neural pathways from the main olfactory bulb. Neuroscience 57:1007-1025[Medline].
3.	Belyavskyi, M., E. Belyavskaya, G. A. Levy, and J. L. Leibowitz. 1998. Coronavirus MHV-3-induced apoptosis in macrophages. Virology 250:41-49[Medline].
4.	Bergmann, C. C., Q. Yao, M. Lin, and S. A. Stohlman. 1996. The JHM strain of mouse hepatitis virus induces a spike protein-specific Db-restricted cytotoxic T cell response. J. Gen. Virol. 77:315-325[Abstract/Free Full Text].
5.	Bond, C. W., J. L. Leibowitz, and J. A. Robb. 1979. Pathogenic murine coronaviruses: II. Characterization of virus-specific proteins of murine coronaviruses JHMV and A59V. Virology 94:371-384[Medline].
6.	Bos, E. C. W., L. Heijnen, W. Luytjes, and W. J. M. Spaan. 1995. Mutational analysis of the murine coronavirus spike protein: effect on cell-to-cell fusion. Virology 214:453-463[Medline].
7.	Castro, R. F., and S. Perlman. 1995. CD8⁺ T-cell epitopes within the surface glycoprotein of a neurotropic coronavirus and correlation with pathogenicity. J. Virol. 69:8127-8131[Abstract].
8.	Collins, A. R., R. L. Knobler, H. Powell, and M. J. Buchmeier. 1982. Monoclonal antibodies to murine hepatitis virus-4 (strain JHM) define the viral glycoprotein responsible for attachment and cell-cell fusion. Virology 119:358-371[Medline].
9.	Compton, S. R., S. W. Barthold, and A. L. Smith. 1993. The cellular and molecular pathogenesis of coronaviruses. Lab. Anim. Sci. 43:15-28[Medline]. [Erratum 43:203.]
10.	Dalziel, R. G., P. W. Lampert, P. J. Talbot, and M. J. Buchmeier. 1986. Site-specific alteration of murine hepatitis virus type 4 peplomer glycoprotein E2 results in reduced neurovirulence. J. Virol. 59:463-471[Abstract/Free Full Text].
11.	Daniel, C., R. Anderson, M. J. Buchmeier, J. O. Fleming, W. J. M. Spaan, H. Wege, and P. J. Talbot. 1993. Identification of an immunodominant linear neutralization domain on the S2 portion of the murine coronavirus spike glycoprotein and evidence that it forms part of complex tridimensional structure. J. Virol. 67:1185-1194[Abstract/Free Full Text].
12.	DeGroot, R. J., W. Luytjes, M. C. Horzinek, B. A. M. van der Zeijst, W. J. M. Spaan, and J. A. Lenstra. 1987. Evidence for a coiled-coil structure in the spike proteins of coronaviruses. J. Mol. Biol. 196:963-966[Medline].
13.	Fazakerley, J. K., S. E. Parker, F. Bloom, and M. J. Buchmeier. 1992. The V5A13.1 envelope glycoprotein deletion mutant of mouse hepatitis virus type-4 is neuroattenuated by its reduced rate of spread in the central nervous system. Virology 187:178-188[Medline].
14.	Fischer, F., C. F. Stegen, C. A. Koetzner, and P. S. Masters. 1997. Analysis of a recombinant mouse hepatitis virus expressing a foreign gene reveals a novel aspect of coronavirus transcription. J. Virol. 71:5148-5160[Abstract].
15.	Fleming, J. O., M. D. Trousdale, F. A. K. El-Zaatari, S. A. Stohlman, and L. P. Weiner. 1986. Pathogenicity of antigenic variants of murine coronavirus JHM seleced with monoclonal antibodies. J. Virol. 58:869-875[Abstract/Free Full Text].
16.	Frana, M. F., J. N. Behnke, L. S. Sturman, and K. V. Holmes. 1985. Proteolytic cleavage of the E2 glycoprotein of murine coronavirus: host-dependent differences in proteolytic cleavage and cell fusion. J. Virol. 56:912-920[Abstract/Free Full Text].
17.	Gallagher, T. M. 1997. A role for naturally occurring variation of the murine coronavirus spike protein in stabilizing association with the cellular receptor. J. Virol. 71:3129-3137[Abstract].
18.	Gallagher, T. M., C. Escarmis, and M. J. Buchmeier. 1991. Alteration of pH dependence of coronavirus-induced cell fusion: effect of mutations in the spike glycoprotein. J. Virol. 65:1916-1928[Abstract/Free Full Text].
19.	Gallagher, T. M., S. E. Parker, and M. J. Buchmeier. 1990. Neutralization-resistant variants of a neurotropic coronavirus are generated by deletions within the amino-terminal half of the spike glycoprotein. J. Virol. 64:731-741[Abstract/Free Full Text].
20.	Gilmore, W., J. O. Fleming, S. A. Stohlman, and L. P. Weiner. 1987. Characterization of the structural proteins of the murine coronavirus strain A59 using monoclonal antibodies. Proc. Soc. Exp. Biol. Med. 185:177-186[Medline].
21.	Gombold, J. L., S. T. Hingley, and S. R. Weiss. 1993. Fusion-defective mutants of mouse hepatitis virus A59 contain a mutation in the spike protein cleavage signal. J. Virol. 67:4504-4512[Abstract/Free Full Text].
22.	Higuchi, R. 1990. PCR protocols: a guide to methods and applications, p. 177-183. Academic Press, Inc., San Diego, Calif.
23.	Hingley, S. T., J. L. Gombold, E. Lavi, and S. R. Weiss. 1994. MHV-A59 fusion mutants are attenuated and display altered hepatotropism. Virology 200:1-10[Medline].
24.	Houtman, J. J., and J. O. Fleming. 1996. Pathogenesis of mouse hepatitis virus-induced demyelination. J. Neurovirol. 2:361-376[Medline].
25.	Koetzner, C. A., M. M. Parker, C. S. Ricard, L. S. Sturman, and P. S. Masters. 1992. Repair and mutagenesis of the genome of a deletion mutant of the murine coronavirus mouse hepatitis virus by targeted RNA recombination. J. Virol. 66:1841-1848[Abstract/Free Full Text].
26.	Kubo, H., Y. K. Yamada, and F. Taguchi. 1994. Localization of neutralizing epitopes and the receptor-binding site within the amino-terminal 330 amino acids of the murine coronavirus spike protein. J. Virol. 68:5403-5410[Abstract/Free Full Text].
26a.	Kuo, L., G.-J. Godeke, M. J. B. Raamsman, P. S. Masters, and P. J. M. Rottier. Retargeting of coronavirus by substitution of the spike glycoprotein ectodomain: crossing the host species barrier. Submitted for publication.
27.	Lane, T. E., H. S. Fox, and M. J. Buchmeier. 1999. Inhibition of nitric oxide synthase-2 reduces the severity of mouse hepatitis virus-induced demyelination: implications for NOS2/NO regulation of chemokine expression and inflammation. J. Neurovirol. 5:48-54[Medline].
28.	Lavi, E., P. S. Fishman, M. K. Highkin, and S. R. Weiss. 1988. Limbic encephalitis after inhalation of a murine coronavirus. Lab. Invest. 58:31-36[Medline].
29.	Lavi, E., D. H. Gilden, M. K. Highkin, and S. R. Weiss. 1986. The organ tropism of mouse hepatitis virus strain A59 is dependent on dose and route of inoculation. Lab. Anim. Sci. 36:130-135[Medline].
30.	Lavi, E., E. M. Murray, S. Makino, S. A. Stohlman, M. M. C. Lai, and S. R. Weiss. 1990. Determinants of coronavirus MHV pathogenesis are localized to 3' portions of the genome as determined by ribonucleic acid-ribonucleic acid recombination. Lab. Invest. 62:570-578[Medline].
31.	Leparc-Goffart, I., S. T. Hingley, M. M. Chua, J. Phillips, E. Lavi, and S. R. Weiss. 1998. Targeted recombination within the spike gene of murine coronavirus mouse hepatitis virus-A59: Q159 is a determinant of hepatotropism. J. Virol. 72:9628-9636[Abstract/Free Full Text].
32.	Lewis, J., S. L. Wesselingh, D. E. Griffin, and J. M. Hardwick. 1996. Alphavirus-induced apoptosis in mouse brains correlates with neurovirulence. J. Virol. 70:1828-1835[Abstract].
33.	Liang, X. H., J. E. Goldman, H. H. Jiang, and B. Levine. 1999. Resistance of interleukin-1B-deficient mice to fatal Sindbis encephalitis. J. Virol. 73:2563-2567[Abstract/Free Full Text].
34.	Luo, Z., and S. R. Weiss. 1998. Roles in cell-to-cell fusion of two conserved hydrophobic regions in the murine coronavirus spike protein. Virology 244:483-494[Medline].
35.	Luytjes, W., L. S. Sturman, P. J. Bredenbeck, J. Charite, B. A. M. van der Zeijst, M. C. Horzinek, and W. J. M. Spaan. 1987. Primary structure of the glycoprotein E2 of coronavirus MHV-A59 and identification of the trypsin cleavage site. Virology 161:479-487[Medline].
36.	Masters, P. S., C. A. Koetzner, C. A. Kerr, and Y. Heo. 1994. Optimization of targeted RNA recombination and mapping of a novel nucleocapsid gene mutation in the coronavirus mouse hepatitis virus. J. Virol. 68:328-337[Abstract/Free Full Text].
37.	Parker, S. E., T. M. Gallagher, and M. J. Buchmeier. 1989. Sequence analysis reveals extensive polymorphism and evidence of deletions within the E2 glycoprotein gene of several strains of murine hepatitis virus. Virology 173:664-673[Medline].
38.	Pope, M., P. A. Marsden, E. Cole, S. Sloan, L. S. Fung, Q. Ning, J. W. Ding, J. L. Leibowitz, M. J. Phillips, and G. A. Levy. 1998. Resistance to murine hepatitis virus strain 3 is dependent on production of nitric oxide. J. Virol. 72:7084-7090[Abstract/Free Full Text].
39.	Ramig, R. F. 1982. Isolation and genetic characterization of temperature sensitive mutants of simian rotavirus SA11. Virology 120:93-135[Medline].
40.	Rao, P. V., and T. M. Gallagher. 1998. Intracellular complexes of viral spike and cellular receptor accumulate during cytopathic murine coronavirus infections. J. Virol. 72:3278-3288[Abstract/Free Full Text].
41.	Reed, L. J., and H. Muench. 1938. A simple method of estimating fifty per cent points. Am. J. Hyg. 27:493-497.
42.	Sasseville, V. G., M. M. Smith, C. R. Mackay, D. R. Pauley, K. G. Mansfield, D. J. Ringler, and A. A. Lackner. 1996. Chemokine expression in simian immunodeficiency virus-induced AIDS encephalitis. Am. J. Pathol. 149:1459-1467[Abstract].
43.	Smith, A. L., and S. W. Barthold. 1997. Methods in viral pathogenesis, p. 483-506. In N. Nathanson (ed.), Viral pathogenesis. Lippincott-Raven, Philadelphia, Pa.
44.	Sturman, L. S., C. S. Ricard, and K. V. Holmes. 1985. Proteolytic cleavage of the E2 glycoprotein of murine coronavirus: activation of cell fusing activity of virions by trypsin and separation of two different 90K cleavage fragments. J. Virol. 56:904-911[Abstract/Free Full Text].
45.	Wege, H., J. Winter, and R. Meyermann. 1988. The peplomer protein E2 of coronavirus JHM as a determinant of neurovirulence: definition of critical epitopes by variant analysis. J. Gen. Virol. 69:87-98[Abstract/Free Full Text].
46.	Williams, R. K., G. S. Jiang, and K. V. Holmes. 1991. Receptor for mouse hepatitis virus is a member of the carcinoembryonic antigen family of glycoproteins. Proc. Natl. Acad. Sci. USA 88:5533-5536[Abstract/Free Full Text].