Genetic Evidence for an Interferon-Antagonistic Function of Rift Valley Fever Virus Nonstructural Protein NSs

doi:10.1128/JVI.75.3.1371-1377.2001

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Journal of Virology, February 2001, p. 1371-1377, Vol. 75, No. 3
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.3.1371-1377.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Genetic Evidence for an Interferon-Antagonistic Function of Rift Valley Fever Virus Nonstructural Protein NSs

Michèle Bouloy,¹ Christian Janzen,²^, Pierre Vialat,¹ Huot Khun,³ Jovan Pavlovic,⁴ Michel Huerre,³ and Otto Haller²^,^*

Groupe des Bunyaviridés¹ and Unité d'Histopathologie,³ Institut Pasteur, F-75724 Paris Cedex, France; Institute of Medical Virology, University of Zürich, CH-8028 Zürich, Switzerland⁴; and Abteilung Virologie, Institut für Medizinische Mikrobiologie und Hygiene, Universität Freiburg, D-79008 Freiburg, Germany²

Received 21 August 2000/Accepted 3 November 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Rift Valley fever virus (RVFV), a phlebovirus of the family Bunyaviridae, is a major public health threat in Egypt and sub-SaharanAfrica. The viral and host cellular factors that contribute toRVFV virulence and pathogenicity are still poorly understood.All pathogenic RVFV strains direct the synthesis of a nonstructuralphosphoprotein (NSs) that is encoded by the smallest (S) segmentof the tripartite genome and has an undefined accessory function.In this report, we show that MP12 and clone 13, two attenuatedRVFV strains with mutations in the NSs gene, were highly virulentin IFNAR^/ mice lacking the alpha/beta interferon (IFN- $alpha$ / $beta$ ) receptor butremained attenuated in IFN- $gamma$ receptor-deficient mice. Both attenuatedstrains proved to be excellent inducers of early IFN- $alpha$ / $beta$ production.In contrast, the virulent strain ZH548 failed to induce detectableamounts of IFN- $alpha$ / $beta$ and replicated extensively in both IFN-competentand IFN-deficient mice. Clone 13 has a defective NSs gene witha large in-frame deletion. This defect in the NSs gene resultsin expression of a truncated protein which is rapidly degraded.To investigate whether the presence of the wild-type NSs genecorrelated with inhibition of IFN- $alpha$ / $beta$ production, we infectedsusceptible IFNAR^/ mice with S gene reassortant viruses. When the S segment of ZH548was replaced by that of clone 13, the resulting reassortants becamestrong IFN inducers. When the defective S segment of clone 13was exchanged with the wild-type S segment of ZH548, the reassortantvirus lost the capacity to stimulate IFN- $alpha$ / $beta$ production. Theseresults demonstrate that the ability of RVFV to inhibit IFN- $alpha$ / $beta$ production correlates with viral virulence and suggest that theaccessory protein NSs is an IFNantagonist.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Alpha/beta interferons (IFNs- $alpha$ / $beta$ ) are key components of the innate immune mechanisms that protect the host against invadingviruses (23, 31, 42). The extraordinary power of the IFNsystem has prompted many viruses to adopt strategies that inhibitIFN production or action (for a review, see reference 13). Wetherefore considered the possibility that virulent strains ofRift Valley fever virus (RVFV) differ from attenuated strainsin their capacity to actively antagonize the IFN response of thehost. RVFV is a mosquito-borne virus which belongs to the Bunyaviridaefamily (Phlebovirus genus). Periodically, the virus causes epidemicsand epizootics in sub-Saharan countries of Africa and in Egypt.In humans, infection leads to a wide spectrum of clinical symptomsthat range from a benign fever to severe encephalitis, retinitis,and fatal hepatitis with hemorrhagic fever (27). Among animals,sheep and goats are severelyaffected.

Like all members of the family, RVFV possesses a single-stranded segmented RNA genome composed of a large (L), a medium (M),and a small (S) segment (for reviews, see references 9, 11,and 40). The L and M segments are of negative polarity. TheL segment codes for the RNA-dependent RNA polymerase. The M segmentcodes for a polyprotein which is the precursor to the glycoproteinsG1 and G2 and two nonstructural proteins, 14K and 78K. The S segmenthas two open reading frames that do not overlap. They code forthe nucleoprotein N and the nonstructural protein NSs in an ambisensecoding strategy. The roles of the nonstructural proteins, in particularthe NSs protein, are stillunknown.

Safe and efficient vaccines for both human and veterinary use are urgently needed. In the past, efforts were undertaken todevelop live attenuated vaccine strains by natural selection fromwild-type strains. Thus, the Smithburn neurotropic strain of RVFVwas derived from the virulent Entebbe strain after numerous intracerebralpassages in mice (41). It is still in use as a veterinary livevirus vaccine, irrespective of its considerable neurotropism,abortogenicity, and teratogenicity. More recently, two additionalattenuated strains, MP12 and clone 13, were obtained. The MP12strain was derived from the virulent Egyptian strain ZH548 (6).Strain ZH548 was originally isolated from the serum of an uncomplicatedhuman febrile case of RVF that occurred during the Egyptian outbreakof 1977 (26). The virus was then propagated for 12 serial tissueculture passages in the presence of the mutagenic agent 5-fluorouracil,generating strain MP12. It was later shown that MP12 carries attenuatingmutations in each genomic segment and was considered a safe vaccine(39). Clone 13 represents an avirulent virus variant that hasa large deletion in the S segment and is naturally attenuated.It was biologically cloned by plaque purification from a fieldisolate obtained from a nonfatal human case during the 1974 RVFoutbreak in Bangui, Central African Republic (30). Clone 13is unique in that it grows well in Vero cells but is avirulentin vivo. It has no pathogenicity for mice or hamsters, in thatthese animals survive large infectious doses of up to 10⁶ PFU without developing any signs of disease. In addition, clone13 is highly immunogenic, leading to long-lasting immunity (30).

Recent work with reassortant viruses demonstrated that the attenuation phenotype is mediated by the S segment of clone 13,which contains a defective NSs gene (45). The wild-type NSsgene codes for a nonstructural protein of 265 amino acids thatis abundantly expressed in infected cells. The NSs gene of clone13 has a large internal in-frame deletion of 549 nucleotides whichremoves 70% of the open reading frame but conserves the N andC termini of the protein. As a consequence, a truncated NSs proteinof 82 amino acids is produced but is rapidly degraded in infectedcells by the proteasome pathway (45). The NSs protein of RVFVis unique among members of the Bunyaviridae family, as it is phosphorylatedand found in the nucleus of infected cells, where it forms largefilamentous structures (21, 47). This nuclear localizationis surprising because RVFV, like all members of the family, replicatesexclusively in the cytoplasm. All attempts to define a role forNSs have failed so far. In experimental reconstitution systems,the protein has neither a stimulatory nor an inhibitory effecton transcription or replication of RVFV (24, 36). The NSs-deficientclone 13 is able to multiply normally in IFN-deficient Vero cellsas well as in mosquito cells or whole Culex pipiens mosquitoes(30). This may suggest that the NSs gene has evolved duringadaptation of RVFV to the mammalian host and that an importantrole of the NSs protein was to provide a mechanism to circumventthe IFN response of vertebrate cells. Using mice which are unableto respond to IFN- $alpha$ / $beta$ or IFN- $gamma$ , we demonstrate that the S segmentof RVFV determines IFN- $alpha$ / $beta$ production in the infected host. Thepresent results suggest that the NSs protein is an important virulencefactor that prevents IFNs- $alpha$ / $beta$ from being induced early duringthe course of RVFVinfection.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Viruses. Virus strains ZH548, MP12 (6), clone 13 (30), and reassortants between ZH548 and clone 13 (45) were propagated in Verocells using a multiplicity of infection (MOI) of 0.001. Viruspresent in the supernatant was usually harvested 3 days afterinfection. Virus titers were determined by plaque assay in Verocells.

Animal studies. IFN-competent mice of inbred strain 129/SvPasIco were obtained from Iffa Credo, Les Oncins, France. Transgenic mice with targeteddisruptions of the $beta$ -subunit of the IFN- $alpha$ / $beta$ receptor (IFNAR^/) or the IFN- $gamma$ receptor (IFNGR^/) on an inbred 129SV/Ev genetic background were bred and raisedas described (16, 19, 31). Age- and sex-matched animalswere inoculated intraperitoneally with 10⁴ PFU of RVFV. Mortality was recorded twice a day. Animals wereobserved for a maximum of 21days.

IFN assay. At various times after infection, venous blood was collected from each group of mice and pooled. The pooled sera were treatedat pH 2 overnight, readjusted to pH 7.2, and stored frozen ( $-$ 72°C)until use. Serum IFN titers were determined in a biological assay,using mouse L929 cells and vesicular stomatitis virus, as describedpreviously (15). IFN titers are expressed as units per milliliterof serum, standardized against a standard preparation of recombinanthuman IFN- $alpha$ B/D (Novartis, Basel, Switzerland) known to be activeon mouse cells (18).

Histopathological examination. Specimens including liver and spleen were fixed in formalin and embedded in paraffin. Serial 5-µm-thick tissue sections werestained with hematoxylin and eosin, periodic acid Schiff, andGordon sweet stains according to the protocols described by Bancroftet al. (2). Immunohistochemical analysis was performed as described(14), using a mouse polyclonal antibody directed against baculovirus-expressednucleoprotein N of RVFV strain MP12. Briefly, tissue sectionswere immersed in 200 ml of citrate and incubated three times for5 min in a microwave oven at 650 W before staining. The alkalinephosphatase method with fast red as a chromogen (LSAB 2 universalalkaline phosphatase kit; Dako, Trappes, France) was used to detectthe secondary antibody. Slides were counterstained with Meyer'shematoxylin. Negative controls included tissue samples obtainedfrom uninfectedmice.

In situ hybridization. A ³⁵S probe was prepared by labeling the EcoRI-cleaved DNA insert of plasmid pBS-N in the presence of [³⁵S]dATP using the random-primed DNA labeling kit (Boehringer, Mannheim,Germany). The pBS-N plasmid contains the N protein sequence ofthe MP12 strain from nucleotides 1008 to 1691 (according to thesequence of the genome strand reported previously [12]) insertedat the unique EcoRI site of the BlueScript polylinker (Stratagene).In situ hybridization was performed as previously described (32).Briefly, deparaffinized slides were dehydrated in a blocking solutionto inhibit nonspecific binding of the probe. The slides were acetylatedin 0.1 M triethanolamine (pH 8) and washed in a solution composedof formamide and 2× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodiumcitrate). The probe containing 5 × 10⁴ cpm/ml was denatured for 2 min at 80°C and incubated for 16 h.The slides were then washed in SSC solution, followed by incubationin a photographic emulsion. Slides were counterstained in Harrishematoxylin and mounted in Eukittmedium.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Attenuated RVFV strains are fully pathogenic for mice lacking a functional IFN- $alpha$ / $beta$ system. It has previously been shown that the virulent strain ZH548 is pathogenic for laboratory mice after intraperitoneal or subcutaneousinoculation, causing acute hepatitis and death of the animalswithin a few days after infection with a dose as low as 10 PFU(45). In contrast, strains MP12 and clone 13 are highly attenuated,as indicated by the fact that mice survive experimental infectionswith virus doses of up to 10⁵ to 10⁶ PFU (6). The mechanisms responsible for this astonishing differencein pathogenicity have not been elucidated. To assess a possiblerole of virus-induced IFN- $alpha$ / $beta$ , we infected genetically modifiedmice defective for the IFN- $alpha$ / $beta$ receptor (IFNAR^/ mice) and appropriate control mice with either the attenuatedstrain MP12, the attenuated strain clone 13, or the virulent strainZH548. Six mice in each group were infected intraperitoneallywith 10⁴ PFU of virus and observed for 21 days. Blood samples were obtainedat various times after infection to monitor viremia and serumIFN- $alpha$ / $beta$ levels. Figure 1 shows that strain ZH548 killed both IFNAR^/ mice and wild-type mice within 4 to 5 days, as expected. IFNAR^/ mice showed an accelerated death rate, indicating that they weresomewhat more susceptible than wild-type mice (Fig. 1A). In contrast,wild-type mice infected with MP12 or clone 13 survived for 21days without any signs of disease, as previously reported (45)(Fig. 1B and C). However, none of the IFNAR^/ mice survived. In fact, all the mice died from the infectionwithin 2 to 3 days. This rapid death was unexpected, as it resembledthat of mice infected with virulent strain ZH548. Therefore, additionalexperiments with MP12 and clone 13 were performed. They gave thesame results and showed that IFNAR^/ mice died very rapidly after infection with virus doses as lowas 10 PFU (data not shown). The 50% lethal dose (LD₅₀) of clone13 was found to be approximately 1 to 5 PFU for IFNAR^/ mice. It thus resembles the LD₅₀ of virulent strain ZH548 forwild-type mice (45).

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FIG. 1. High virulence of attenuated RVFV strains in IFN-deficient mice. IFNAR^/ mice lacking the receptor for IFN- $alpha$ / $beta$ (solid triangles) and genotype-matched normal mice (open circles) were infected intraperitoneally with 10⁴ PFU of either wild-type virus ZH548 (A), attenuated strain MP12 (B), or attenuated strain clone 13 (C). Survival was assessed daily for up to 21 days.

To investigate whether IFN- $gamma$ plays a comparable role in mediating in vivo attenuation of RVFV strains, mice having a targetedmutation inactivating the IFN- $gamma$ receptor were infected with 10⁴ PFU of attenuated virus strain MP12 or clone 13. IFNAR^/ mice and wild-type mice were included in these experiments assusceptible and resistant controls, respectively. All six IFNGR^/ mice survived infection without showing disease symptoms, asdid the six wild-type mice, whereas all six of the IFNAR^/ mice succumbed to infection with either strain. These resultsclearly demonstrate that IFN- $gamma$ plays at best a negligible rolein RVFV attenuation but that IFN- $alpha$ / $beta$ is absolutely required forsurvival.

Attenuated strains cause fulminant hepatitis in IFNAR^/ mice. To assess the cause of death due to infection with the attenuated viruses in IFNAR^/ mice, histopathological examinations were performed. On postmortem examination of mice inoculated with clone 13, a swollenand congested liver was most prominent. Microscopically, the liversexhibited the salient features associated with RVFV infection(25, 29). The mice showed signs of a fulminant hepatitis withcentrolobular, mostly perivascular coagulative necrosis and massivedestruction of the whole lobules except for a layer of hepatocytesaround the portal area. In these areas, numerous apoptotic nucleiwere detectable (Fig. 2A). Polymorphonuclear or lymphocytic infiltrateswere absent, indicating a rapid onset and fulminant course ofthe destructive process. Staining for glycogen revealed a lossof glycogen from infected livers (Fig. 2C1) compared to controllivers (Fig. 2C2), indicating fresh lesions of acute hepatitis.

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FIG. 2. Fulminant hepatitis caused by attenuated clone 13 in IFN-deficient mice. Histology, immunostaining, and in situ hybridization of post mortem liver sections from IFNAR^/ mice inoculated with 10⁴ PFU of clone 13. (A) Hematoxylin-eosin staining showing perivascular coagulative necrosis and numerous apoptotic nuclei around the portal area. (B) Immunostaining for viral N protein. (C) Loss of glycogen as revealed by periodic acid Schiff staining. (D) In situ hybridization detecting virus-specific nucleic acids in infected (D1) or uninfected (D2) hepatocytes. Magnifications: (A and C) ×360; (B) ×90; (inset) ×225; (D) ×225.

In addition, immunohistochemistry with a monospecific antibody directed against the viral N protein was performed. Infectedhepatocytes were most prominently detected in the perivascularareas but extended into the whole lobule, as demonstrated by strongimmunostaining (Fig. 2B). These hepatocytes were heavily infected,as revealed by the presence of large amounts of viral antigenin the cytoplasm (insert in Fig. 2B). Finally, in situ hybridizationwith an S segment-specific probe demonstrated that numerous hepatocytescontained virus-specific nucleic acids (RNA) in infected (Fig.2D1) but not in uninfected (Fig. 2D2) livers. In the spleen, immunohistochemistryand in situ hybridization confirmed the presence of infected cellsand demonstrated that the macrophages of the perifollicular areasare the main target of the virus (data not shown). These histopathologicalfeatures were identical to those observed in livers and spleensof wild-type mice inoculated with virulent strain ZH548 (datanotshown).

Rapid growth of attenuated RVFV strains in IFNAR^/ mice. Next, we determined the kinetics and extent of virus growth in wild-type and IFNAR^/ mice infected intraperitoneally with 10⁴ PFU of RVFV strain ZH548, MP12, or clone 13 (Fig. 3). The developmentand degree of viremia were assessed by titrating infectious virusin serum samples obtained at various times after infection. ZH548caused a high level of viremia in both normal and IFN-deficientmice (Fig. 3A). Clearly, virus growth was faster and reached 100-fold-highertiters in IFNAR^/ mice compared to control mice. In contrast, both attenuated virusstrains were unable to cause viremia in the IFN-competent wild-typemice (Fig. 3B and C). Obviously, virus multiplication was severelyrestricted, and the infecting virus was unable to reach the bloodstreamin detectable amounts. This lack of viral spread correspondedwell with the absence of overt clinical disease and gross pathologicalchanges in these animals.

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FIG. 3. Attenuated RVFV strains cause viremia in IFN-deficient mice. Growth of virulent virus ZH548 (A), attenuated strain MP12 (B), and attenuated strain clone 13 (C) in IFNAR^/ mice (solid triangles) and control mice (open circles). Serum samples were collected from six mice per group at the indicated times after infection with 10⁴ PFU and pooled before plaque titration on Vero cells.

Interestingly, both MP12 and clone 13 showed a completely different behavior than wild-type virus in the IFNAR^/ mice. High virus titers were detectable with MP12 in sera collected48 h after infection (Fig. 3B). Surprisingly, clone 13 virus grewextremely fast and reached titers of 10⁷ PFU/ml of serum within 28 h (Fig. 3C). In IFN-deficient mice,this otherwise attenuated virus seemed to be even more virulentthan strain ZH548. The rapid viral growth correlated well withthe rapid progression of disease and the early death observedin these animals (Fig. 1C).

Virulent strains are poor inducers of IFN- $alpha$ / $beta$ . Given these findings, it was clear that IFN- $alpha$ / $beta$ was the key player responsible for the attenuation phenotype observed withMP12 and clone 13 in normal mice. We investigated IFN- $alpha$ / $beta$ productionby determining the amount of acid-stable IFN- $alpha$ / $beta$ in aliquots ofthe serum samples used for virus titrations. Figure 4A shows thatIFN- $alpha$ / $beta$ was barely detectable in serum samples from mice infectedwith the virulent strain ZH548. This was unexpected, given theextensive virus multiplication in these animals (Fig. 3A). Interestingly,the MP12 and clone 13 viruses induced large amounts of IFN- $alpha$ / $beta$ in IFNAR^/ mice that were easily detectable in late serum samples (Fig.4B and C). The time course of IFN production correlated well withthe rapid virus growth in these IFN-nonresponsive mice, indicatingthat both viruses are good inducers of IFN- $alpha$ / $beta$ . Significantly,serum IFN was also detectable in normal wild-type mice early inthe course of infection with clone 13 (Fig. 4C). This is remarkablebecause no viremia was present, again indicating that the attenuatedstrain was able to induce an early production of IFN- $alpha$ / $beta$ thatwas restricting further virus growth in the IFN-competent animals.This early IFN peak is likely to be responsible for the attenuationphenotype of clone 13 and possibly MP12 in normal mice. Remarkably,it is not detectable in mice infected with the virulent strainZH548 (Fig. 4A), despite extensive virus replication (Fig. 3A).

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FIG. 4. Virulent RVFV strain ZH548 is a poor inducer of IFN- $alpha$ / $beta$ . Aliquots of the pooled serum samples described in Fig. 3 were inactivated at low pH and tested for acid-stable IFN- $alpha$ / $beta$ in a standard bioassay. Sera were from IFNAR^/ mice (solid triangles) or control mice (open circles) infected with 10⁴ PFU of either wild-type virus ZH548 (A), attenuated strain MP12 (B), or attenuated strain clone 13 (C).

S segment of RVFV controls IFN induction. Clone 13 carries a large in-frame deletion of the NSs gene, which is encoded by the S segment of the tripartite genome. Thisdeletion leads to a truncated and abnormal NSs protein (45).Genetic reassortment between virulent ZH548 and attenuated clone13 demonstrated that the altered S segment carries a major virulence/attenuationdeterminant (45). It was conceivable that this genetic alterationwas also responsible for the increased IFN- $alpha$ / $beta$ production. Toinvestigate this possibility, we used these reassortant virusesand their parental strains to infect IFNAR^/ mice. The reassortant virus carrying the L and M segments ofstrain ZH548 and the defective S segment of clone 13 was namedZ/Z/C. Conversely, the reassortant carrying the intact S segmentof ZH548 in a clone 13 genetic background was called C/C/Z. Groupsof six IFNAR^/ mice were infected with 10⁴ PFU of either wild-type virus ZH548 (Z/Z/Z), mutant clone 13(C/C/C), or the reassortant virus Z/Z/C or C/C/Z. Individual bloodsamples were collected at the indicated times after infection.Sera were pooled within each group, and aliquots were assayedin parallel for infectious virus and IFN- $alpha$ / $beta$ . Figure 5 shows thatthe virulent Z/Z/Z virus grew to high titers and killed the animalswithin 48 h of infection, but it did not induce detectable levelsof IFN- $alpha$ / $beta$ . When the S segment of ZH548 was replaced by that ofclone 13, the resulting Z/Z/C virus also grew to high titers,but it strongly induced IFN synthesis. Likewise, clone 13 (C/C/C)grew well and induced large amounts of IFN- $alpha$ / $beta$ . In contrast, reassortantC/C/Z had lost its capacity to induce IFN- $alpha$ / $beta$ , although it maintainedthe growth characteristics of clone 13. These results formallydemonstrate that the S segment of RVFV carries determinants thatinfluence IFN- $alpha$ / $beta$ production in the infected host. They furthersuggest that the NSs protein targets the IFN- $alpha$ / $beta$ system of thehost but is otherwise not required for efficient virus growth.Taken together, the present results strongly suggest that theIFN response governed by NSs determines viral virulence or attenuationin normal hosts.

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FIG. 5. S segment of RVFV determines IFN inducibility. IFNAR^/ mice were infected with 10⁴ PFU of either wild-type virus ZH548 (Z/Z/Z), attenuated clone 13 (C/C/C), or the reassortant virus Z/Z/C or C/C/Z. Individual blood samples were collected at the indicated times after infection. Sera from six mice per group were pooled, and aliquots were assayed in parallel for infectious virus in a plaque assay (solid triangles) and for IFN- $alpha$ / $beta$ in a standard bioassay (open circles).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The function of the nonstructural protein NSs of RVFV during infection is still unknown. It is a matter of great interest,because the phosphoprotein accumulates in large amounts in thenucleus of infected cells, whereas virus replication takes placeexclusively in the cytoplasm. The nuclear localization of NSsis compatible with the view that NSs is not directly involvedin virus growth but may serve an accessory function. Here we provideevidence suggesting that the main role of the NSs protein of RVFVis to inhibit the IFN response of the host by blocking virus-inducedIFN- $alpha$ / $beta$ production. The evidence is based on a classical geneticapproach, combining genetic modification of the virus with geneticmanipulation of thehost.

We show that the NSs-expressing ZH548 virus is highly virulent and grows to high titers in laboratory mice without inducingdetectable amounts of IFN- $alpha$ / $beta$ , whereas the NSs-defective clone13 virus is an excellent IFN inducer and is highly attenuatedin IFN-responsive mice. The mutant virus shows restored growthand wild-type virulence in genetically altered mice that are nonresponsiveto IFN- $alpha$ / $beta$ . The growth and virulence of the NSs-defective virusare not restored in genetically altered mice that have a defectin the IFN- $gamma$ system. This specific phenotypic restoration clearlyidentifies the IFN- $alpha$ / $beta$ system as the target of NSs. Finally, weshow that a reassortant ZH548 virus with the NSs-defective S segmentof clone 13 becomes a phenocopy of clone 13, and vice versa: areassortant clone 13 virus containing the intact S segment ofthe virulent strain is now a poor IFN inducer but replicates efficientlyin IFN-competent mice. These results demonstrate for the firsttime that the S segment of RVFV carries determinants that regulateIFN- $alpha$ / $beta$ production in the infected host. However, these resultsdo not formally prove that NSs is the responsible factor. Comparisonsof the S segment sequences of clone 13 and ZH548 show that thereare a few changes in addition to the large deletion in the NSsgene, namely, one amino acid change in the N protein sequence(glycine versus glutamic acid at position 159) and six nucleotidechanges in the intergenic region (30, 45). It is highly unlikelythat these differences rather than the loss of NSs function areresponsible for the different phenotypes described here. However,a definitive answer will have to await the availability of recombinantviruses with targeted deletions in the NSs gene. A reverse geneticssystem exists for Bunyamwera virus, another member of the Bunyaviridaefamily (5). A recent report describes a recombinant Bunyamweravirus that lacks NSs and exhibits an attenuation phenotype inmice (A. Bridgen, J. K. Fazakerley, and R. M. Elliott, Abstr.11th Int. Cong. Virol. abstr. VW47.06, 1999). Interestingly, thisNSs-minus virus seems to have gained IFN-inducing properties,indicating that the NSs protein of Bunyamwera virus may also haveIFN-antagonistic functions (F. Weber, A. Bridgen, and R. M. Elliott,Abstr. 11th Int. Conf. Negative-Strand Viruses, abstr. 117,2000).

The MP12 strain of RVFV was derived from strain ZH548 by serial tissue culture passages and cloning in the presence of 5-fluorouracil,a mutagenic substance. The close genetic relationship betweenthe two virus strains allows a direct comparison of their sequences(46). The S segment of MP12 has acquired one nucleotide exchangein the intergenic region and three exchanges in the NSs codingregion, leading to a single-amino-acid substitution from valineto alanine at position 513. This point mutation occurred earlyin the course of passaging, when reduced virulence and reductionin plaque size of the resulting virus was first observed (39,46). It is therefore conceivable that this mutation is responsiblefor the attenuated phenotype observed. However, MP12 acquiredadditional attenuating mutations in the other gene segments duringsubsequent passages in tissue culture (43). Unlike its parentalstrain, the attenuated MP12 proved to be a good IFN inducer inthe present experiments. Moreover, it exhibited virulence in IFNAR^/ mice, exactly like clone 13. It can therefore be assumed thatthe point mutation in NSs acquired during attenuation of MP12inactivates the anti-IFN function of the protein. Alternatively,some of the other attenuating mutations may contribute to thephenotype.

The present results clearly show that both attenuated RVFV strains are fully competent to replicate and to display their inherentpathogenic potential in IFN- $alpha$ / $beta$ -insensitive mice, leading to severedisease and death within a few days after infection. In fact,clone 13 was even more virulent than wild-type strain ZH548, indicatingthat a functional NSs protein is totally dispensable for virusgrowth and pathogenicity in these animals. However, in the presenceof a competent IFN response, these viruses grew poorly and wereapathogenic. It was conceivable that the attenuated viruses werenot only better IFN inducers, as shown here, but were also moresensitive to the antiviral action of IFNs than the pathogenicstrains. We tested this hypothesis using virus-permissive Verocells and recombinant human IFN- $alpha$ , but were unable to detect significantdifferences in IFN sensitivity between MP12, clone 13, and ZH548(data not shown). This is in agreement with a previous study reportingthat RVFV strains that differed in virulence for rats were equallysensitive to the antiviral effect of recombinant human IFN- $alpha$ (1).We conclude that the virulence of a given RVFV strain is not dictatedby its IFN sensitivity but resides in its capacity to efficientlyblock the production of IFN- $alpha$ / $beta$ .

The present findings are not without precedent. An early study by Higashihara and coworkers found that less virulent RVFVstrains were generally more potent IFN- $alpha$ / $beta$ inducers in mice thanthe corresponding more virulent strains (17). Avirulent strainswere able to induce a first peak of IFN at a very early stageof infection, whereas virulent strains were unable to do so buthad circulating IFN later on shortly before death, when the animalshad a high viremia (17). Likewise, Peters and coworkers concludedfrom extensive studies that the outcome of RVFV infections inrodents and monkeys is controlled by early IFN- $alpha$ / $beta$ (1, 28,29, 33, 34).

Most viruses must multiply and spread in the presence of IFNs that activate innate host defense mechanisms. Many viruses seemtherefore to have evolved specific means that circumvent the IFNresponse of the host (for a review, see reference 13). Suchstrategies are especially important for RNA viruses. During theirlife cycle, RNA viruses produce large amounts of double-strandedRNA (dsRNA) which, by itself, is an excellent inducer of IFN- $alpha$ / $beta$ (20). It is therefore not surprising that most negative-strandRNA viruses seem to code for accessory proteins that subvert IFNproduction and/or action (13). A major strategy for blockingIFN- $alpha$ / $beta$ production is to provide a virally encoded dsRNA-bindingprotein that sequesters dsRNA molecules and prevents them frominducing IFN- $alpha$ / $beta$ (10). The sequestration of dsRNA is expectedto reduce the dsRNA-dependent activation of a number of antiviralproteins, including PKR (4, 7, 22), which is also involvedin efficient induction of IFN- $alpha$ / $beta$ (8). A variety of additionalstrategies have been found to operate in different viruses. Forexample, some viruses encode proteins inhibiting the activitiesof cellular transcription factors mediating IFN- $alpha$ / $beta$ induction,such as NF- $kappa$ B (35, 37) and members of the IFN-regulatory factorfamily (3, 37, 38, 44). Given the plethora of mechanismsthrough which NSs could work, it will be interesting to determinewhich strategy is used byRVFV.

	ACKNOWLEDGMENTS

We thank Agnes Billecocq, Jason Paragas, Michael Frese, Georg Kochs, Peter Staeheli, and Adolfo Garcia-Sastre for stimulatingdiscussions and critically reading themanuscript.

This work was supported in part by grant HA 1582 from the DeutscheForschungsgemeinschaft.

	FOOTNOTES

^* Corresponding author. Mailing address: Abteilung Virologie, Institut für Medizinische Mikrobiologie und Hygiene, UniversitätFreiburg, D-79008 Freiburg, Germany. Phone: 49-761-2036534. Fax:49-761-2036626. E-mail: HALLER{at}UKL.UNI-FREIBURG.DE.

Present address: The Rockefeller University, New York, NY10021.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Anderson, G. W., Jr., and C. J. Peters. 1988. Viral determinants of virulence for Rift Valley fever (RVF) in rats. Microb. Pathog. 5:241-250[CrossRef][Medline].

2. Bancroft, J. D., H. C. Cook, R. W. Stirling, and D. R. Turner. 1994. Manual of histological technics and their diagnostic applications. Churchill Livingstone, London, U.K.

3. Barnard, P., and N. A. McMillan. 1999. The human papillomavirus E7 oncoprotein abrogates signaling mediated by interferon-alpha. Virology 259:305-313[CrossRef][Medline].

4. Bergmann, M., A. Garcia-Sastre, E. Carnero, H. Pehamberger, K. Wolff, P. Palese, and T. Muster. 2000. Influenza virus NS1 protein counteracts PKR-mediated inhibition of replication. J. Virol. 74:6203-6206[Abstract/Free Full Text].

5. Bridgen, A., and R. M. Elliot. 1996. Rescue of a segmented negative-stranded RNA virus entirely from cloned complementary DNAs. Proc. Natl. Acad. Sci. USA 93:15400-15404[Abstract/Free Full Text].

6. Caplen, H., C. J. Peters, and D. H. L. Bishop. 1985. Mutagen-directed attenuation of Rift Valley fever virus as a method for vaccine development. J. Gen. Virol. 66:2271-2277[Abstract/Free Full Text].

7. Chang, H. W., J. C. Watson, and B. L. Jacobs. 1992. The E3L gene of vaccinia virus encodes an inhibitor of the interferon-induced, double-stranded RNA-dependent protein kinase. Proc. Natl. Acad. Sci. USA 89:4825-4829[Abstract/Free Full Text].

8. Chu, W. M., D. Ostertag, Z. W. Li, L. Chang, Y. Chen, Y. Hu, B. Williams, J. Perrault, and M. Karin. 1999. JNK2 and IKKbeta are required for activating the innate response to viral infection. Immunity 11:721-731[CrossRef][Medline].

9. Elliott, R. M. (ed.). 1996. The bunyaviridae. Plenum Press, New York, N.Y.

10. Garcia-Sastre, A., A. Egorov, D. Matassov, S. Brandt, D. E. Levy, J. E. Durbin, P. Palese, and T. Muster. 1998. Influenza A virus lacking the NS1 gene replicates in interferon-deficient systems. Virology 252:324-330[CrossRef][Medline].

11. Giorgi, C. 1996. Molecular biology of phleboviruses, p. 105-128. In R. M. Elliott (ed.), The bunyaviridae. Plenum Press, New York, N.Y.

12. Giorgi, C., L. Accardi, L. Nicoletti, M. C. Gro, K. Takehara, C. Hilditch, S. Morikawa, and D. H. Bishop. 1991. Sequences and coding strategies of the S RNAs of Toscana and Rift Valley fever viruses compared to those of Punta Toro, Sicilian sandfly fever, and Uukuniemi viruses. Virology 180:738-753[CrossRef][Medline].

13. Goodbourn, S., L. Didcock, and R. E. Randall. 2000. Interferons: cell signalling, immune modulation, antiviral response and virus countermeasures. J. Gen. Virol. 81:2341-2364[Free Full Text].

14. Hall, W. C., T. P. Crowell, D. M. Watts, V. L. Barros, H. Kruger, F. Pinheiro, and C. J. Peters. 1991. Demonstration of yellow fever and dengue antigens in formalin-fixed paraffin-embedded human liver by immunohistochemical analysis. Am. J. Trop. Med. Hyg. 45:408-417.

15. Haller, O., H. Arnheiter, I. Gresser, and J. Lindenmann. 1979. Genetically determined, interferon-dependent resistance to influenza virus in mice. J. Exp. Med. 149:601-612[Abstract/Free Full Text].

16. Hefti, H. P., M. Frese, H. Landis, C. Di Paolo, A. Aguzzi, O. Haller, and J. Pavlovic. 1999. Human MxA protein protects mice lacking a functional alpha/beta interferon system against La Crosse virus and other lethal viral infections. J. Virol. 73:6984-6991[Abstract/Free Full Text].

17. Higashihara, M., H. Koyama, and Y. Igarashi. 1972. Induction of virus-inhibiting factor or interferon in mice by strains with different virulence of Rift Valley fever virus. Kitasato Arch. Exp. Med. 45:33-43[Medline].

18. Horisberger, M. A., and K. de Staritzky. 1987. A recombinant human interferon-alpha B/D hybrid with a broad host-range. J. Gen. Virol. 68:945-948[Abstract/Free Full Text].

19. Huang, S., W. Hendriks, A. Althage, S. Hemmi, H. Bluethmann, R. Kamijo, J. Vilcek, R. M. Zinkernagel, and M. Aguet. 1993. Immune response in mice that lack the interferon-gamma receptor. Science 259:1742-1745[Abstract/Free Full Text].

20. Jacobs, B. L., and J. O. Langland. 1996. When two strands are better than one: the mediators and modulators of the cellular responses to double-stranded RNA. Virology 219:339-349[CrossRef][Medline].

21. Kohl, A., V. di Bartolo, and M. Bouloy. 1999. The Rift Valley fever virus nonstructural protein NSs is phosphorylated at serine residues located in casein kinase consensus motifs in the carboxy-terminus. Virology 263:517-525[CrossRef][Medline].

22. Langland, J. O., S. Pettiford, B. Jiang, and B. L. Jacobs. 1994. Products of the porcine group C rotavirus NSP3 gene bind specifically to double-stranded RNA and inhibit activation of the interferon-induced protein kinase PKR. J. Virol. 68:3821-3829[Abstract/Free Full Text].

23. Leib, D. A., M. A. Machalek, B. R. Williams, R. H. Silverman, and H. W. Virgin. 2000. Specific phenotypic restoration of an attenuated virus by knockout of a host resistance gene. Proc. Natl. Acad. Sci. USA 97:6097-6101[Abstract/Free Full Text].

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1.	Anderson, G. W., Jr., and C. J. Peters. 1988. Viral determinants of virulence for Rift Valley fever (RVF) in rats. Microb. Pathog. 5:241-250[CrossRef][Medline].
2.	Bancroft, J. D., H. C. Cook, R. W. Stirling, and D. R. Turner. 1994. Manual of histological technics and their diagnostic applications. Churchill Livingstone, London, U.K.
3.	Barnard, P., and N. A. McMillan. 1999. The human papillomavirus E7 oncoprotein abrogates signaling mediated by interferon-alpha. Virology 259:305-313[CrossRef][Medline].
4.	Bergmann, M., A. Garcia-Sastre, E. Carnero, H. Pehamberger, K. Wolff, P. Palese, and T. Muster. 2000. Influenza virus NS1 protein counteracts PKR-mediated inhibition of replication. J. Virol. 74:6203-6206[Abstract/Free Full Text].
5.	Bridgen, A., and R. M. Elliot. 1996. Rescue of a segmented negative-stranded RNA virus entirely from cloned complementary DNAs. Proc. Natl. Acad. Sci. USA 93:15400-15404[Abstract/Free Full Text].
6.	Caplen, H., C. J. Peters, and D. H. L. Bishop. 1985. Mutagen-directed attenuation of Rift Valley fever virus as a method for vaccine development. J. Gen. Virol. 66:2271-2277[Abstract/Free Full Text].
7.	Chang, H. W., J. C. Watson, and B. L. Jacobs. 1992. The E3L gene of vaccinia virus encodes an inhibitor of the interferon-induced, double-stranded RNA-dependent protein kinase. Proc. Natl. Acad. Sci. USA 89:4825-4829[Abstract/Free Full Text].
8.	Chu, W. M., D. Ostertag, Z. W. Li, L. Chang, Y. Chen, Y. Hu, B. Williams, J. Perrault, and M. Karin. 1999. JNK2 and IKKbeta are required for activating the innate response to viral infection. Immunity 11:721-731[CrossRef][Medline].
9.	Elliott, R. M. (ed.). 1996. The bunyaviridae. Plenum Press, New York, N.Y.
10.	Garcia-Sastre, A., A. Egorov, D. Matassov, S. Brandt, D. E. Levy, J. E. Durbin, P. Palese, and T. Muster. 1998. Influenza A virus lacking the NS1 gene replicates in interferon-deficient systems. Virology 252:324-330[CrossRef][Medline].
11.	Giorgi, C. 1996. Molecular biology of phleboviruses, p. 105-128. In R. M. Elliott (ed.), The bunyaviridae. Plenum Press, New York, N.Y.
12.	Giorgi, C., L. Accardi, L. Nicoletti, M. C. Gro, K. Takehara, C. Hilditch, S. Morikawa, and D. H. Bishop. 1991. Sequences and coding strategies of the S RNAs of Toscana and Rift Valley fever viruses compared to those of Punta Toro, Sicilian sandfly fever, and Uukuniemi viruses. Virology 180:738-753[CrossRef][Medline].
13.	Goodbourn, S., L. Didcock, and R. E. Randall. 2000. Interferons: cell signalling, immune modulation, antiviral response and virus countermeasures. J. Gen. Virol. 81:2341-2364[Free Full Text].
14.	Hall, W. C., T. P. Crowell, D. M. Watts, V. L. Barros, H. Kruger, F. Pinheiro, and C. J. Peters. 1991. Demonstration of yellow fever and dengue antigens in formalin-fixed paraffin-embedded human liver by immunohistochemical analysis. Am. J. Trop. Med. Hyg. 45:408-417.
15.	Haller, O., H. Arnheiter, I. Gresser, and J. Lindenmann. 1979. Genetically determined, interferon-dependent resistance to influenza virus in mice. J. Exp. Med. 149:601-612[Abstract/Free Full Text].
16.	Hefti, H. P., M. Frese, H. Landis, C. Di Paolo, A. Aguzzi, O. Haller, and J. Pavlovic. 1999. Human MxA protein protects mice lacking a functional alpha/beta interferon system against La Crosse virus and other lethal viral infections. J. Virol. 73:6984-6991[Abstract/Free Full Text].
17.	Higashihara, M., H. Koyama, and Y. Igarashi. 1972. Induction of virus-inhibiting factor or interferon in mice by strains with different virulence of Rift Valley fever virus. Kitasato Arch. Exp. Med. 45:33-43[Medline].
18.	Horisberger, M. A., and K. de Staritzky. 1987. A recombinant human interferon-alpha B/D hybrid with a broad host-range. J. Gen. Virol. 68:945-948[Abstract/Free Full Text].
19.	Huang, S., W. Hendriks, A. Althage, S. Hemmi, H. Bluethmann, R. Kamijo, J. Vilcek, R. M. Zinkernagel, and M. Aguet. 1993. Immune response in mice that lack the interferon-gamma receptor. Science 259:1742-1745[Abstract/Free Full Text].
20.	Jacobs, B. L., and J. O. Langland. 1996. When two strands are better than one: the mediators and modulators of the cellular responses to double-stranded RNA. Virology 219:339-349[CrossRef][Medline].
21.	Kohl, A., V. di Bartolo, and M. Bouloy. 1999. The Rift Valley fever virus nonstructural protein NSs is phosphorylated at serine residues located in casein kinase consensus motifs in the carboxy-terminus. Virology 263:517-525[CrossRef][Medline].
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