Noncytopathic Bovine Viral Diarrhea Virus Inhibits Double-Stranded RNA-Induced Apoptosis and Interferon Synthesis

doi:10.1128/JVI.75.10.4692-4698.2001

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Journal of Virology, May 2001, p. 4692-4698, Vol. 75, No. 10
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.10.4692-4698.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Noncytopathic Bovine Viral Diarrhea Virus Inhibits Double-Stranded RNA-Induced Apoptosis and Interferon Synthesis

Matthias Schweizer^* and Ernst Peterhans

Institute of Veterinary Virology, University of Bern, CH-3012 Bern, Switzerland

Received 14 September 2000/Accepted 23 February 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Bovine viral diarrhea virus (BVDV), a pestivirus of the Flaviviridae family, is an economically important cattle pathogenwith a worldwide distribution. Both noncytopathic (ncp) and cytopathic(cp) biotypes of BVDV can be isolated from persistently infectedcattle suffering from the lethal mucosal disease. The cp biotypecorrelates with the production of the NS3 nonstructural protein,which in the corresponding ncp biotype is present in its uncleavedform, NS23. Previously, we have shown that cp but not ncp BVDVinduces the formation of $alpha$ / $beta$ interferons in bovine macrophages.In this study, we demonstrate that ncp BVDV inhibits the inductionof apoptosis and the expression of interferon $alpha$ / $beta$ by poly(IC),a synthetic double-stranded RNA (dsRNA). Inhibition was observedonly in cells which had been infected with ncp BVDV at least 12h prior to the addition of dsRNA, which indicates that expressionof viral proteins is necessary for the ncp virus to inhibit theeffects of poly(IC). Additional experiments using transfectedpoly(IC) showed that ncp BVDV interfered with the intracellularaction of dsRNA rather than with its uptake into the cells. Infectedcells were not resistant to induction of apoptosis by actinomycinD or staurosporine, which suggests that ncp BVDV may specificallyinterfere with signaling through dsRNA. Interference with theinnate antiviral host responses may explain the successful establishmentof persistent infection by ncp BVDV in fetuses early in theirdevelopment.

	INTRODUCTION

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To establish a persistent infection, a virus must overcome the defense mechanisms of both the innate and the specific immuneresponses. Antigenic changes, latency, and replication in immunologicallyprivileged sites permit the viruses to escape the effects of Tcells and antibodies (4, 10, 20). Viral mechanisms directedagainst the innate immune system target, among others, the host'scytokine response and the complement system (4, 51, 68).Apoptosis and the interferon (IFN) response are important antiviraldefense mechanisms that act at the level of the host cells. Thefact that these mechanisms may be triggered hours to days beforethe onset of the virus-specific immune response highlights theirrole as a first line of defense. Moreover, as apoptosis and theIFN response are a characteristic of virtually all cells of metazoananimals, they help the host to fight a broad range of viruseswith different cell and tissue tropisms. It is no surprise, therefore,that viruses have evolved a myriad of mechanisms that preventapoptosis and subvert the IFN response. In the past few years,several viral gene products with antiapoptotic or anti-IFN activitieshave been identified and described in extensive reviews (15,18, 51, 57, 62, and references therein). These strategiesinclude modulation of the Bcl-2/Bax pathway, interference withcaspases, a group of proteases known to be part of the death effectormechanism of apoptosis, or inhibition of the PKR/RNase Lpathway.

Bovine viral diarrhea virus (BVDV), together with classical swine fever and border disease viruses of sheep, belongs to thegenus Pestivirus of the Flaviviridae family. BVDV is an economicallyimportant cattle pathogen with a worldwide distribution. The viruscauses acute (transient) and persistent infections. Cattle infectedacutely with BVDV may show either no symptoms or mild diarrhea(caused by "avirulent" BVDV strains), but severe thrombocytopeniaand hemorrhages have also been reported (virulent strains) (42,66). According to their effect in cell cultures, cytopathic(cp) and noncytopathic (ncp) biotypes of BVDV can be isolated.Infection of pregnant animals with the ncp biotype may resultin embryo death, resorption, and stillbirth and induce nonfatalteratogenic damage or may lead to the birth of persistently infectedcalves. Such calves are immunotolerant to the infecting BVDV strainand remain viremic for the rest of their lives. Such persistentlyinfected animals are predisposed to infections with other pathogensand run a high risk of developing the fatal mucosal disease whichis characterized by extensive lesions in the gastrointestinaltract (43, 46, 66, and references therein). From animalssuccumbing to mucosal disease, both an ncp and an antigenicallyrelated cp BVDV can be isolated; they are hence referred to asa virus pair (11). The cp biotype may arise in persistentlyinfected animals by genomic rearrangement of the ncp virus, e.g.,insertion of cellular sequences or rearrangements in the viralgenome (for reviews, see references 42 and 53). In every casestudied so far, the genomic changes leading to the cp biotypeare paralleled by the production of the nonstructural proteinNS3(p80).

Previously, we reported that cp BVDV induce the synthesis of IFN- $alpha$ / $beta$ (IFN type I) in infected macrophages (1, 50) andkill their host cells by apoptosis (59, 72). By contrast,ncp biotypes of BVDV do not induce the synthesis of IFN, and cellsshow no signs of viral infection, even though the viral titersproduced by cp and ncp virus pairs may be similar. In this paper,we show that cells infected with ncp BVDV resist cell death anddo not form IFN in response to the synthetic double-stranded RNA(dsRNA) poly(IC). Resistance to the potent proapoptotic and IFN-inducingeffects of dsRNA may be a key factor in the successful invasionof the fetus and lifelong persistence of thevirus.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Reagents. Fetal calf serum (FCS) and cell culture media were purchased from Seromed (Biochrom, Munich, Germany). FCS was free of BVDVand antibody to BVDV as tested by virus isolation and serum neutralizationassays, respectively. Synthetic polyribonucleotides [polyinosinic-polycytidylicacid, poly(IC); polyadenylic-polyuridylic acid, poly(AU); polycytidylicacid, poly(C); and polyinosinic acid, poly(I)] and staurosporinewere from Sigma. Actinomycin D was from Alexis Corporation (Läufelfingen,Switzerland). All other chemicals were of the highest purity commerciallyavailable.

Cells and viruses. Primary bovine turbinate (BT) cells were prepared from fetuses obtained from a local abattoir and maintained in minimal essentialmedium supplemented with 7% FCS (2% FCS after viral infection),penicillin (100 IU/ml), and streptomycin (100 µg/ml) at 37°C ina humidified 5% CO₂ atmosphere. MDBK cells were obtained fromthe American Type Culture Collection (Manassas, Va.) and maintainedunder the same conditions as the BT cells. Monocyte-derived macrophages(M $phi$ ) were obtained from the blood of Red Holstein cows as describedpreviously (31). All cells were found to be free of BVDV byimmunofluorescence testing. The TGAC (54) and SuwaCP cp BVDVstrains and the TGAN (54), SD-1, SuwaNCP, R6229/95, R5013/96,and 890 ncp viruses were used (all strains are of BVDV genotypeI except for strain 890, which belongs to genotype II). Strains890, R6229/95, and R5013/96 are virulent strains, whereas allother strains are avirulent. The TGAC and TGAN virus strains werekindly provided by V. Moennig (Hannover, Germany), and strain890 was kindly provided by J. F. Ridpath (Ames, Iowa), whereasSuwaCP, SuwaNCP, R6229/95, and R5013/96 are virus strains isolatedat our institute. SuwaCP and SuwaNCP are a virus pair isolatedfrom an animal with mucosal disease (50), and R6229/95 and R5013/96are from acutely infected animals showing thrombocytopenia andhemorrhages. Vesicular stomatitis virus (VSV) (strain Indiana)was kindly provided by H. Hengartner, Institute of ExperimentalImmunology, Zurich, Switzerland. Viruses were passaged and titratedon BT cells as described (2), and the titer of the virus stockswas calculated according to Reed and Muench (52).

Virus infection. BT cells seeded in microwell plates (96 wells) or six-well plates at a density of 10⁶ (microwell plate) or 1.2 × 10⁶ (six-well plate) cells/plate were infected with the appropriateBVDV strain in a small volume of culture medium without FCS ata multiplicity of infection (MOI) of 1 for 1 h at 37°C. Afteradsorption of the virus, the inoculum was removed by washing thecells in culture medium without FCS prior to the addition of completemedium with 2% FCS. Using an MOI of 1, expression of NS3 or NS23was detectable at 6 h postinfection by Western blot or immunohistochemistry,and all cells expressed NS3/NS23 around 12 to 18 h postinfection,as analyzed by immunofluorescence staining using an anti-NS3/NS23antibody.

DNA fragmentation. The fragmentation of cellular DNA was analyzed quantitatively by fluorescence-activated cell sorting (FACS) analysis accordingto Cossarizza et al. (16). Briefly, adherent and detached cellswere collected by centrifugation at 250 × g and washed in phosphate-bufferedsaline (PBS), and the cell pellet (10⁵ cells) was lysed in 250 µl of 0.1 M sodium citrate (pH 6.5)-1%Triton X-100-10 µg of propidium iodide (PI) per ml. Nuclei wereanalyzed after a 30-min incubation at 4°C in the dark with a FACScanflow cytometer (Becton Dickinson, San José, Calif.), and a minimumof 10⁴ nuclei wereanalyzed.

Measurement of the cellular redox state. The cellular redox state was analyzed by determination of the oxidation of dichlorofluorescin to the fluorescent dichlorofluorescein(DCF) and FACS analysis as described (12). Adherent and detachedcells were collected as described above and resuspended in 500µl of PBS. After addition of 10 µM 2',7'-dichlorodihydrofluoresceindiacetate (Kodak, Rochester, N.Y.), cells were incubated for 30min at 37°C in the dark, followed immediately by FACS analysis.To separate viable and dead cells, PI (final concentration, 10µg/ml) was added 10 min prior to the end of the incubation. Cellfluorescence was analyzed with a FACScan flow cytometer, withthe fluorescence of DCF analyzed in channel 1 (FL1; log scale)and that of PI in channel 2 (FL2; log scale). A minimum of 10⁴ cells per sample were analyzed, and the oxidation state (geometricmean) of the viable cells was calculated by gating for the cellsexcluding PI, which cannot pass through the intact plasma membrane.For comparison of the different samples, preparations were recordedat single instrument amplificationsettings.

IFN- $alpha$ / $beta$ activity. Procedures for measuring biological activity of IFN- $alpha$ / $beta$ in supernatants of virus-infected cells have been described previously.The assay used is based on the reduction of Sendai virus growthby IFN- $alpha$ / $beta$ contained in $beta$ -propiolactone-inactivated cell culturesupernatants as determined by immunocytochemistry (49). Fortransfection of cells with poly(IC) to induce IFN- $alpha$ / $beta$ , Lipofectin(Gibco Life-Technologies AG, Basel, Switzerland) at 8 µg/ml wasused according to the manufacturer's protocol. Briefly, Lipofectinwas incubated at room temperature in serum- and antibiotic-freemedium for 45 min before mixing with poly(IC). The Lipofectin-poly(IC)mixture was incubated another 15 min at room temperature beforebeing added to the cells. After incubation for 2 h, the inoculumwas replaced by fresh medium containing 2%FCS.

RT-PCR and Southern blot analysis. Reverse transcription (RT)-PCR and Southern blot analysis were performed with slight modifications according to Sager et al.(58). Briefly, cells were harvested from 25 cm² culture flasks, and total RNA was isolated with Trizol (GibcoLife Technologies) according to the manufacturer's protocol. RNA(10 µg) was adjusted to 0.1 µg/µl and treated with DNase I (4U/µg of RNA) (Boehringer, Mannheim, Germany) in the presence ofRNasin (8 U/µg of RNA) (Promega, Madison, Wis.) for 2 h at 37°C.After purification of the DNA-free RNA by phenol-chloroform extraction,RT was performed for 2 h at 42°C in the presence of oligo(dT)primers and 10 U of avian myeloblastosis virus reverse transcriptase(AMV-RT) (Promega) in a total volume of 100 µl. To exclude amplificationfrom contaminating IFN- $alpha$ / $beta$ DNA which escaped DNase treatment,a negative control without the addition of AMV-RT was included.Five microliters of the RT product was used in the following PCR.The primers used were specific for subfamilies of IFN ( $alpha$ , $beta$ , $omega$ ,and $gamma$ ), and glyceraldehyde-3-phosphate dehydrogenase (GAPDH)-specificprimers were included as a loading control. A temperature profileof 1 min at 94°C, 1 min at 55°C, and 1 min at 72°C after "hotstart" addition of Taq polymerase was used for 30 cycles. Thesequences of the IFN-specific primers used for the PCR have beendescribed (58).

Southern blotting was performed by transferring the amplified material from the agarose gel onto a positively charged nylonmembrane (Boehringer Mannheim). The material was cross-linkedby heat treatment at 80°C for 2 h. Prehybridization for 4 h andhybridization overnight with digoxigenin (DIG)-labeled RNA probesspecific for IFN- $alpha$ , - $beta$ , - $omega$ , and - $gamma$ and GAPDH was performed at50°C. The hybridized blot was washed several times in 2× SSC (1×SSC is 0.15 M NaCl plus 0.015 M sodium citrate, pH 7)-0.1% sodiumdodecyl sulfate (SDS) and in 0.1× SSC-0.1% SDS at room temperatureand at 68°C, according to the manufacturer's protocol (BoehringerMannheim). Staining was done with anti-DIG-alkaline phosphataseconjugate (Boehringer Mannheim) and CDP-Star (Tropix, Bedford,Mass.) as substrate. A high-performance autoradiography film (Hyperfilm-MP;Amersham, Buckinghamshire, U.K.) was exposed for 2 to 30s.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell death induced by dsRNA is inhibited by ncp BVDV. Addition of poly(IC), a synthetic dsRNA mimic, to BT cells resulted in cell death in a concentration-dependent manner, asshown by PI staining of the nuclei and FACS analysis (Fig. 1A).Accordingly, the double-stranded oligonucleotide poly(AU) alsoinduced cell death at 10 to 500 µg/ml, albeit less efficientlythan poly(IC) (not shown). By contrast, BT cells which had previouslybeen infected with ncp BVDV were fully protected from cell deathinduced by poly(IC) (Fig. 1A) or poly(AU) (not shown), even atthe highest concentration tested. The single-stranded oligonucleotidespoly(I) and poly(C) did not induce cell death in either mock-infected(Fig. 1B) or ncp BVDV-infected BT cells (not shown). However,when poly(I) and the complementary poly(C) were added simultaneouslyto the cells, they induced cell death, albeit less efficientlythan poly(IC) (Fig. 1B), which was again completely inhibitedin ncp BVDV-infected cells (not shown). When poly(I) and poly(C)were incubated before addition to BT cells, they induced celldeath as efficiently as poly(IC) (not shown), confirming thatthe dsRNA moiety is important for induction of apoptosis. By contrast,cell death induced by staurosporine, an inhibitor of protein kinaseC and a widely used apoptosis inducer, or by actinomycin D, aninhibitor of cellular transcription (70), was not inhibitedby infecting BT cells with ncp BVDV (not shown).

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FIG. 1. Ncp BVDV inhibits cell death induced by dsRNA in BT cells. BT cells in six-well plates were either mock infected or infected with the TGAN ncp BVDV strain at an MOI of 1 at 18 h prior to the addition of the oligonucleotides (A and B). DNA fragmentation was analyzed 48 h later by PI staining of nuclei followed by FACS analysis as described in the text. The percentages on the y axis indicate nuclei with subgenomic DNA. (A) Mock- (

) or TGAN-infected ( $open circle$ ) BT cells were treated with poly(IC) at the indicated concentrations (mean ± standard deviation [SD], n = 4 to 13). (B) Mock-infected BT cells were treated with poly(IC) (

), poly(I) and poly(C) at equal concentrations (

), poly(I) ( $black-triangle$ ), or poly(C) ( $triangle$ ) at the indicated concentrations (mean ± SD, n = 2 to 6). (C) BT cells were mock- (

) or TGAN- (

, $open circle$ ) infected 6 h (

, $open circle$ ) and 12 h (

) prior to the addition of poly(IC), and DNA fragmentation was analyzed 48 h later. For clarity, the mean ± SD (n = 2 to 3) is shown only for cells infected for 6 h. For mock-infected cells, the SD is similar for both time points, and for cells infected by TGAN for 12 h, the SD is smaller than the symbols.

Protein expression is necessary for BVDV to inhibit dsRNA-induced cell death. To test whether the expression of viral proteins is necessary for protection from dsRNA-induced apoptosis, we infected BTcells with ncp BVDV at 0, 6, 12, or 24 h prior to the additionof poly(IC). Ncp BVDV did not protect cells from apoptosis whenadded simultaneously with poly(IC) (not shown), whereas infectionof BT cells 6 and 12 h prior to poly(IC) addition partially orfully protected BT cells from poly(IC)-induced cell death, respectively(Fig. 1C). This clearly shows that expression of viral or cellularproteins induced by the virus is necessary for the inhibitoryactivity of ncp BVDV-infected BTcells.

Apoptosis-inhibiting activity is independent of the virus strain used. Recent analysis identified two major BVDV genotypes, called BVDV-I and BVDV-II (48). Most outbreaks of severe disease aftertransient infections were associated with BVDV-II, but it is nowevident that virulent ncp BVDV strains exist in both genotypes(9). We tested several strains of either BVDV-I or -II andavirulent or virulent ncp BVDV strains to analyze whether theability to inhibit dsRNA-induced cell death differs between differentgenotypes or between strains of different virulence. All ncp BVDVstrains tested, i.e., the avirulent TGAN, SuwaNCP, and SD-1 andthe virulent R6229/95 and R5013/96 strains of genotype I and the890 BVDV-II strain, completely inhibited cell death induced bypoly(IC) at up to 500 µg/ml (notshown).

ROS are not involved in dsRNA-induced cell death. We have previously shown that intracellular oxidative stress is a crucial step in the induction of apoptosis induced by cpBVDV (59). To analyze whether cell death induced by both poly(IC)and cp BVDV requires the production of reactive oxygen species(ROS) and whether ncp BVDV would inhibit such an increase in ROS,we measured the intracellular redox state by quantitating theoxidation of dichlorofluorescin to the fluorescent DCF by FACSanalysis (59). In contrast to the TGAC cp BVDV strain, poly(IC)at up to 500 µg/ml did not induce intracellular production ofROS in either mock- or ncp BVDV-infected BT cells (Fig. 2).

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FIG. 2. Poly(IC) does not induce the production of ROS in BT cells. BT cells were either mock infected or infected with the TGAN ncp BVDV strain and incubated for 18 h at 37°C. Thereafter, poly(IC) at 0, 50, 100, or 500 µg/ml (groups of bars from left to right) was added, or BT cells were infected with the TGAC cp BVDV strain (single solid bar). The intracellular redox state was measured 24 h later by quantitation of DCF fluorescence of viable, PI-negative cells by flow cytometry as described in the text. The value (geometric mean) for mock-infected cells in the absence of poly(IC) was set at 100% (mean ± SD, n = 2 to 3).

Inhibition of IFN synthesis. It has been known for a long time that dsRNA, e.g., poly(IC), stimulates the production of IFN- $alpha$ / $beta$ (69). Therefore, we wereinterested in whether infection by ncp BVDV, besides protectingfrom cell death, also inhibits the production of IFN induced bydsRNA. As was previously shown (58), uninfected bovine monocyte-derivedM $phi$ produced IFN- $alpha$ / $beta$ in response to poly(IC) (Fig. 3A), as measuredby the reduction in Sendai virus replication. By contrast, IFNsynthesis induced by poly(IC) was completely inhibited in ncpBVDV-infected M $phi$ . The production of IFN- $alpha$ / $beta$ in supernatants ofcp BVDV-infected M $phi$ was enhanced by the addition of poly(IC) (Fig.3A). To exclude the possibility that infection by ncp BVDV merelyinhibits the uptake of poly(IC), we transfected poly(IC) intothe cells using the liposome Lipofectin (47). Poly(IC) at 1µg/ml in the presence of Lipofectin strongly induced the productionof IFN- $alpha$ / $beta$ from MDBK cells, which was completely inhibited inncp BVDV-infected cells (Fig. 3B). Neither unstimulated MDBK cellsnor the addition of Lipofectin alone or poly(IC) at 20 µg/ml inthe absence of Lipofectin induced the production of IFN- $alpha$ / $beta$ inncp BVDV-infected or uninfected MDBK cells. This strongly suggeststhat proteins expressed inside ncp BVDV-infected cells were requiredto inhibit the effects of intracellular dsRNA.

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FIG. 3. Production of IFN- $alpha$ / $beta$ activity is inhibited by ncp BVDV. (A) Bovine monocyte-derived M $phi$ were either mock infected or infected with the TGAN ncp or TGAC cp BVDV strain and incubated for 18 h at 37°C. Thereafter, the M $phi$ were incubated for 4 h in medium with (

) or without (

) poly(IC) (50 µg/ml), followed by 18 h in fresh medium in the absence of poly(IC). The IFN- $alpha$ / $beta$ activity in the supernatants was determined as described in the text. The value for mock-infected cells in the absence of poly(IC) was set at 100% (mean ± SD, n = 3). (B) MDBK cells were either mock infected (

, left bars) or infected with the TGAN ncp BVDV strain (

, right bars) and incubated for 18 h at 37°C. Thereafter, poly(IC) (1 µg/ml) plus Lipofectin (LF) (8 µg/ml) or poly(IC) (20 µg/ml) in the absence of Lipofectin was added as described in the text. Medium (mock) or Lipofectin alone was added as a negative control. The IFN- $alpha$ / $beta$ activity in the supernatants was determined after 24 h as described above and expressed as the standard (recboIFN $alpha$ I.1), that corresponded to the biological activity measured for the sample.

Inhibition of IFN mRNA synthesis. To test whether the inhibition of IFN synthesis occurs at the level of transcription, we analyzed the expression of IFN mRNAby RT-PCR followed by Southern blotting. The primers used werespecific for the different bovine IFN families, i.e., IFN- $alpha$ , - $omega$ ,and - $beta$ (IFN type I) or IFN- $gamma$ (IFN type II), as described in Materialsand Methods. Mock-infected monocyte-derived M $phi$ showed low expressionof mRNA for IFN- $alpha$ , - $omega$ , and - $beta$ , but not IFN- $gamma$ (Fig. 4, lane 1).The expression of all IFN- $alpha$ / $beta$ but not IFN- $gamma$ mRNAs was enhancedby treating the M $phi$ with poly(IC) (Fig. 4, lane 2). By contrast,ncp BVDV-infected M $phi$ did not express or only barely expressedmRNA for either IFN- $alpha$ / $beta$ or IFN- $gamma$ whether stimulated by poly(IC)or unstimulated (Fig. 4, lanes 3 and 4). Surprisingly, M $phi$ culturesinfected with cp BVDV showed strong induction of IFN- $gamma$ mRNA (Fig.4, lanes 5 and 6), even when the blood-derived monocytes wereisolated from cows which were BVDV antibody negative. However,since we never detected IFN- $gamma$ mRNA in bone marrow-derived M $phi$ (3;M. Schweizer, unpublished data), we believe that a cell type differentfrom M $phi$ , e.g., lymphocytes, present in the cultures may be responsiblefor the expression of IFN- $gamma$ mRNA. PCR products obtained withoutprevious addition of RT showed no bands after hybridization withthe specific probes, indicating that no genomic DNA was amplified(not shown).

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FIG. 4. Expression of IFN- $alpha$ / $beta$ mRNA is inhibited by ncp BVDV. Monocyte-derived M $phi$ were mock infected (lanes 1 and 2) or infected by the TGAN ncp (lanes 3 and 4) or TGAC cp BVDV strain (lanes 5 and 6) 18 h prior to the addition of poly(IC) (50 µg/ml) (lanes 2, 4, and 6). After stimulation for 4 h, M $phi$ were incubated for 18 h in fresh medium in the absence of poly(IC). Total RNA was isolated, and IFN mRNA was analyzed by RT-PCR and Southern blotting as described in the text. M $phi$ , which were infected with bovine herpesvirus I were used as positive controls (+) for IFN- $alpha$ / $beta$ (including IFN- $omega$ ), and Theileria parva-transformed cells served as positive controls for IFN- $gamma$ . GAPDH mRNA was included as a loading control.

Antiviral activity of IFN- $alpha$ / $beta$ is not inhibited. Since NS5A of hepatitis C virus (HCV) (another member of the Flaviviridae family) has been shown to inhibit the antiviralactivity of IFN- $alpha$ (24), we tested whether intact BVDV inhibitsnot only the induction but also the activity of IFN- $alpha$ / $beta$ . WhenVSV was used as the challenge virus, recombinant bovine IFN- $alpha$ I.1 at between 10 and 100 ng/ml completely inhibited virus replicationin mock-infected BT cells and fully blocked the cytopathic effect(CPE) induced by VSV, as measured by FACS analysis. Infectionof BT cells by ncp BVDV 18 h prior to the addition of IFN didnot inhibit its antiviral activity (not shown). Thus, the replicationof VSV and the CPE proceeded as in mock-infected cells, and IFNcompletely abolished these effects. This shows that ncp BVDV inhibitsthe induction of IFN- $alpha$ / $beta$ by dsRNA, but it does not inhibit itsantiviral activity when IFN is addedexogenously.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

dsRNA is formed during the multiplication of most viruses and is an important trigger for apoptosis and IFN synthesis (14,30, 32, 35, 37, 69). This study shows that ncp BVDVinhibits apoptosis and IFN mRNA and protein synthesis inducedby poly(IC), a synthetic form of dsRNA. This effect is specificto dsRNA, since (i) poly(AU)-induced cell death was also inhibitedin ncp BVDV-infected cells, and (ii) cell death induced by staurosporineor by actinomycin D was not inhibited by infection with ncp BVDV.The latter is in contrast to poliovirus, a small positive-strandRNA virus of the genus Enterovirus in the Picornaviridae family,which was reported to inhibit actinomycin D- or cycloheximide-inducedapoptosis in HeLa cells (67), or to NIH 3T3 cells expressinga carboxy-terminally truncated NS3 protein of HCV, which weremore resistant to apoptosis induced by actinomycin D (22).

A number of reports suggest that triggering and execution of virus-induced apoptosis and of IFN synthesis may have commonpathways. Specifically, IFN- $alpha$ / $beta$ were shown to be essential mediatorsor to potentiate apoptotic cell death in virus-infected cells(6, 64). Evidence is accumulating that PKR, an enzyme activatedby dsRNA and involved in the induction of IFN synthesis as wellas the in the manifestation of its antiviral activity, may beequally important in triggering apoptosis in virally infectedcells (25, 32, 63). Further strengthening the close correlationbetween the two key mechanisms of antiviral defense is the factthat IFN action and apoptosis are defective in mice devoid of2',5'-oligoadenylate-dependent RNase L (73). This enzyme isresponsible for degrading single-stranded viral RNA, and its apoptosis-promotingeffect may be explained by degradation of cellular mRNA (13,36).

The observations reported in this paper indicate that ncp BVDV may be added to the growing list of viruses that interferewith apoptosis and IFN induction, two mechanisms that are fundamentalto the host defense against viruses at the level of individualcells. Infection with Ebola virus was shown to suppress poly(IC)-inducedsynthesis of several proteins involved in antiviral defense, e.g.,major histocompatibility complex I, 2',5'-oligoadenylate synthetase,and PKR (28). More directly targeting dsRNA, the NS1 proteinof influenza A virus (8, 38), the E3L protein of severalpoxviruses, and the $sigma$ 3 protein of reovirus (57 and referencestherein) were demonstrated to bind to dsRNA and to inhibit theactivation of PKR or RNaseL.

The precise mechanisms by which BVDV interferes with apoptosis and IFN synthesis remain to be elucidated. The possibilitythat ncp BVDV may merely inhibit the uptake of poly(IC), e.g.,by downregulating its receptor (71), was excluded by transfectingdsRNA using Lipofectin (Figure 3B). The inhibition of apoptosisand IFN production depended on the synthesis of BVDV proteins,a feature different from the particle-bound IFN-suppressing activityof VSV Indiana serotypes (40). The core protein of HCV, a flavivirusclosely related to BVDV in its genome structure, has been reportedto be immunosuppressive and to inhibit apoptosis, but the resultsare contradictory (19, 34, and references therein). The HCVE2 protein was reported to inhibit PKR by sequence homology tothe PKR and eIF2 $alpha$ phosphorylation sites (65), and NS5A inhibitspoly(IC)-induced apoptosis (24) and the antiviral activity ofIFN by directly interacting with PKR (23, 33, 60). In theabsence of suitable cell culture systems, it is, however, unknownwhether these effects, observed by expressing individual viralproteins, are also operative during viral multiplication. Additionally,as suggested by experiments in which all viral proteins were jointlyexpressed, PKR-independent mechanisms of interference with apoptosisand IFN action may exist (5, 21). However, using intact virus,we showed that infection of BT cells by ncp BVDV prior to theaddition of IFN did not inhibit its antiviral activity, i.e.,exogenously added IFN- $alpha$ inhibited the replication and cytopathogenicityof VSV independently of infection byBVDV.

It is noteworthy that the BVDV proteins homologous to those found to have antiapoptotic and anti-IFN properties in HCV areidentical in both cp and ncp BVDV. This suggests that if E2 andNS5A are involved in the antiapoptotic and anti-IFN activitiesof BVDV, their roles would be rather complex. The two biotypesdiffer in only one nonstructural protein, which is present inncp BVD V-infected cells in its uncleaved form, NS23, whereasthis protein is cleaved into NS2 and NS3 in cells infected withthe cp biotype of BVDV (11, 42). Since infectious progenyare formed to similar titers in a given pair of ncp and cp BVDV,the NTPase, RNA helicase, and protease activities of this nonstructuralprotein (26, 27) appear to be preserved in the cp biotypeof BVDV. However, as noted previously, the amount of viral RNApresent in cells infected by cp BVDV may vastly exceed that incells infected with ncp biotypes of BVDV (41; L. Perler andH. P. Stalder, unpublished data). This suggests that cp BVDV maybe relatively inefficient at packaging viral RNA compared to itsncp counterpart. Accordingly, RNA replicons of classical swinefever virus lacking the NS2 gene replicated more efficiently andinduced CPE, in contrast to replicons expressing the completeNS23 gene (44). Additionally, the replication of flaviviruses,including BVDV, is known to involve replicative intermediatesand replicative forms of virus RNA (53). Therefore, dsRNA canbe expected to be produced during the replication of cp as wellas ncp BVDV. It is tempting to speculate that a large amount ofviral RNA may be double-stranded, which would have implicationsboth for the cytopathic and interferon-inducing properties ofcp BVDV. This would not necessarily ascribe the evasion by ncpBVDV of apoptosis and IFN induction solely to altered functionof the viral helicase after cleavage of NS23 into NS2 and NS3.In fact, while the presence of NS3 (specifically its N-terminalpart) clearly correlates with the cytopathic properties of BVDV,the cleavage of NS23 may have implications for the function ofother proteins of the replicationcomplex.

It is not only the viral mechanisms for inducing or preventing apoptosis that are different; the biochemical pathways of apoptosismay also vary in virally infected cells (57 and references therein).We have recently demonstrated evidence of oxidative stress incells infected with cp BVDV. Supporting a causative role for thischange, we were able to protect cells from apoptosis by treatmentwith selected antioxidants (59). The fact that we noted no evidenceof oxidative stress in cells undergoing apoptosis in responseto poly(IC) (Fig. 2) argues against a simple correlation betweencell death induced by dsRNA and by cp BVDV. It does not, however,rule out a role of dsRNA in cp BVDV-inducedapoptosis.

The experiments reported in this paper shed new light on observations made some 20 years ago when the capacity to suppressan effect of poly(IC) was used to detect ncp BVDV. Thus, cellswere inoculated with serial dilutions of imput ncp BVDV, treatedwith poly(IC), and subsequently challenged with VSV. Noninfectedcells were found to be protected against VSV-induced CPE, whereasncp BVDV-infected cells were not protected (39). However, theauthors suggested a non-IFN-based mechanism for the antiviralactivity of poly(IC), since in their experiments, ncp BVDV didnot interfere with the production of IFN by poly(IC) (55). Thereason for this difference from the findings reported in thispaper is not clear. The authors of that study observed that certaincell types were unsuitable for their assay of ncp BVDV (56).However, we used different cell types in our study, i.e., BT cells,MDBK cells, and M $phi$ , and a variety of different virus strains,which strongly suggests that interference with dsRNA-induced apoptosisand IFN synthesis by ncp BVDV may indeed be a general and importantactivity of thisvirus.

As shown by many examples, interference with apoptosis and the IFN response may contribute significantly to the success ofviruses in the interaction with their hosts. In some instances,this has been correlated with virulence, i.e., the degree of viralpathogenicity. For example, increased induction of apoptosis hasbeen correlated with attenuation of Sendai virus (29), and wild-typemeasles virus was shown to suppress the induction of IFN- $alpha$ / $beta$ inphytohemagglutinin-stimulated peripheral blood lymphocytes, whichwas lost upon attenuation of the virus in cell culture (45).We observed that all ncp BVDV strains tested avoided apoptosisand IFN induction, i.e., virulent strains reported to induce hemorrhagesin acutely infected animals as well as avirulent strains wereactive. This difference from other viruses may explain why transmissionto the fetus is apparently correlated with the biotype (ncp versuscp) of BVDV rather than with the capacity to cause clinical signsin pregnant animals. Transmission at an early stage of pregnancyis essential for the establishment of immunological toleranceto BVDV (66). As apoptosis and the IFN response are manifestedfrom the earliest stages of pregnancy (61), evasion of thesetwo key elements of the innate immune system may be crucial notonly for transmission to the fetus, but also for the maintenanceof immunotolerance (7, 17, and referencestherein).

	ACKNOWLEDGMENTS

This work was supported by the Swiss National Science Foundation, grant 31-50745.97.

We thank C. Dubey for help with the RT-PCR and Southern blot analysis, H. Pfister for performing the assays for IFN- $alpha$ / $beta$ activity,and R. Parham for critically reading themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Veterinary Virology, University of Bern, Laenggass-Str. 122, CH-3012 Bern,Switzerland. Phone: 41 (31) 631 24 97. Fax: 41 (31) 631 25 34.E-mail: schweizer{at}ivv.unibe.ch.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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