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Recovery of genetically defined murine norovirus in tissue culture by using a fowlpox virus expressing T7 RNA polymerase

¹ Calicivirus Research Group, Department of Virology, Faculty of Medicine, Imperial College London, St Mary's Campus, Norfolk Place, London W2 1PG, UK
² Vaccine Vector Group, Department of Virology, Faculty of Medicine, Imperial College London, St Mary's Campus, Norfolk Place, London W2 1PG, UK

Correspondence
Ian G. Goodfellow
I.Goodfellow{at}imperial.ac.uk

	ABSTRACT

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Despite the significant disease burden caused by human norovirus infection, an efficient tissue-culture system for these viruses remains elusive. Murine norovirus (MNV) is an ideal surrogate for the study of norovirus biology, as the virus replicates efficiently in tissue culture and a low-cost animal model is readily available. In this report, a reverse-genetics system for MNV is described, using a fowlpox virus (FWPV) recombinant expressing T7 RNA polymerase to recover genetically defined MNV in tissue culture for the first time. These studies demonstrated that approaches that have proved successful for other members of the family Caliciviridae failed to lead to recovery of MNV. This was due to our observation that vaccinia virus infection had a negative effect on MNV replication. In contrast, FWPV infection had no deleterious effect and allowed the recovery of infectious MNV from cells previously transfected with MNV cDNA constructs. These studies also indicated that the nature of the 3'-terminal nucleotide is critical for efficient virus recovery and that inclusion of a hepatitis delta virus ribozyme at the 3' end can increase the efficiency with which virus is recovered. This system now allows the recovery of genetically defined noroviruses and will facilitate the analysis of the effects of genetic variation on norovirus pathogenesis.

Published online ahead of print on 25 April 2007 as DOI 10.1099/vir.0.82940-0.

A supplementary table showing details of oligonucleotides used during this study is available with the online version of this paper.

	INTRODUCTION

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Positive-strand RNA viruses of the family Caliciviridae are responsible for many diseases in both man and animals. Those that infect humans, namely members of the genera Norovirus and Sapovirus, are a major cause of acute gastroenteritis and are thought to be responsible for >85 % of all non-bacterial gastroenteritis outbreaks in Europe between 1995 and 2000 (Lopman et al., 2003).

The calicivirus positive-sense, single-strand RNA genome is approximately 7.5 kb in length, encodes three open reading frames and is linked covalently to the virus-encoded protein VPg (Fig. 1a). During virus replication, a subgenomic RNA is produced, encoding the major and minor capsid proteins VP1 and VP2, respectively (Fig. 1a). Despite the major disease burden that caliciviruses cause, we know little with regard to how these viruses replicate and, hence, the identification of potential antivirals and therapeutics has been hindered. This is primarily due to the fact that the human caliciviruses do not replicate efficiently in tissue culture. Although recent reports have demonstrated genome replication and encapsidation by using a vaccinia virus (VACV) expression system (Asanaka et al., 2005; Katayama et al., 2006), the mechanism of synthesis of this RNA and whether it represents authentic VPg-linked viral RNA are still not known. The subgenomic RNA produced from a full-length cDNA clone in one of these systems is not translated, suggesting that it is not VPg-linked (Katayama et al., 2006). A recent report would also suggest that cell lines containing a Norwalk virus replicon can be generated at low frequency (Chang et al., 2006). This lack of an efficient, fully permissive tissue-culture system for human noroviruses has slowed the analysis of the molecular mechanisms used for norovirus genome translation and replication.

View larger version (23K): [in this window] [in a new window]   Fig. 1. Diagrammatic representation of the MNV genome and the constructs used during this study. (a) Proteolytic-cleavage map of the MNV 1 genome as demonstrated by Sosnovtsev et al. (2006). Text in italics highlights the nomenclature as proposed by Sosnovtsev et al. (2006). The caspase 3 cleavage sites in NS1/2 and the position of the subgenomic RNA are also indicated. (b) Schematic representation of the constructs used during this study. The positions of the restriction sites used during this study, the active site in the viral RNA-dependent RNA polymerase NS7 and the 3'-terminal nucleotide upstream of the poly-A tail are indicated. See Methods for specific details of each construct.

	METHODS

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Materials.
MNV 1 strain CW1, the murine macrophage line RAW 264.7 and antisera to the MNV VP1 protein were kindly supplied by Herbert Virgin IV (Washington University in Saint Louis, MO, USA). MVA-T7 (Wyatt et al., 1995) was kindly supplied by Bernie Moss (NIH, Bethesda, MA, USA). Rabbit polyclonal antisera to the MNV NS7 RNA-dependent RNA polymerase and VP2 proteins were generated against proteins expressed in and purified from Escherichia coli as poly-histidine-tagged proteins (data not shown). Both NS7 and VP2 were purified under denaturing conditions (8 M urea) on nickel agarose and used for immunization of New Zealand White rabbits. All immunizations and test bleeds were carried out by Eurogentec.

All cells were maintained in Dulbecco's modified Eagle's medium (Gibco) containing 10 % fetal calf serum. The Huh 7.5 cell line was kindly provided by Charlie Rice (Rockefeller University, NY, USA). The BSR-T7 cell line was obtained from Karl-Klaus Conzelmann (Ludwig Maximilians University, Munich, Germany).

Generation of MNV expression constructs.
A full-length cDNA clone of MNV 1 CW1 matching the passage 3 consensus sequence (Wobus et al., 2004), referred to as p20.3 by Sosnovtsev et al. (2006), was supplied by Herbert Virgin IV (Washington University in Saint Louis, MO, USA). For clarity, this construct, containing the MNV 1 genome under the control of a truncated T7 RNA polymerase promoter, will be hereafter referred to as pT7 : MNV-G. A derivative of this construct (pT7 : MNV-G^FS), containing a frame shift in the RNA-dependent RNA polymerase [NS7 in Fig. 1(a)], was generated by linearization with XhoI, followed by mung-bean nuclease digestion and religation. A transfer vector containing the AfeI–SacII fragment of the MNV-1 genome (pSL301 : MNV AfeI–SacII) was generated by cloning the fragment into pSL301 (Invitrogen). To repair the frame-shift mutation in pT7 : MNV-G^FS, the AfeI–SacII fragment from the transfer vector pSL301 : MNV AfeI–SacII was inserted into pT7 : MNV-G^FS to generate pT7 : MNV-G^FS/R.

A BglII restriction site was introduced at position 3959 in the MNV genome by the introduction of a single-nucleotide change (C to A) at position 3959 to generate pT7 : MNV-G/BglII. The restriction site was introduced by PCR amplification of the region using the primers IGIC44 and 4450R (See Supplementary Table S1, available in JGV Online), digestion with AfeI and KpnI and subsequent insertion into the pSL301 : MNV AfeI–SacII transfer vector (see above). The mutated fragment was subcloned into pT7 : MNV-G via the AfeI and SacII sites. Insertion of the desired mutation, which did not affect the encoded polypeptide sequence, was confirmed by sequencing.

To insert a hepatitis delta virus ribozyme into pT7 : MNV-G at the 3' end of the genome and to repair the 3'-terminal nucleotide, a derivative of the ribozyme containing a 5' NheI site was PCR-amplified from pRZ (Walker et al., 2003) using the primers PUC-F and PUC-R (see Supplementary Table S1, available in JGV Online). The resultant PCR product was digested with NheI and ligated to the NheI-digested MNV subgenomic PCR product generated by using primers IGIC21 and IGIC37 (see Supplementary Table S1, available in JGV Online). The ligated product was subsequently digested with SacII and EcoRV and inserted into pT7 : MNV-G that had been digested with SacII and SnaBI. The resultant plasmid, pT7 : MNV-G 3'Rz, contained the MNV genomic RNA flanked by a truncated T7 RNA polymerase promoter at the 5' end and a hepatitis delta virus ribozyme at the 3' end. The RNA produced from this construct contained no additional non-viral nucleotides. A similar construct that lacked the 3' ribozyme, but which contained a correct 3'-terminal nucleotide, referred to as pT7 : MNV-G 3'Rp, was generated by ligation of the 3' SacII–NheI fragment from pT7 : MNV-G 3'Rz with SacII- and SnaBI-digested pT7 : MNV. The resulting construct, pT7 : MNV-G 3'Rp, was identical to pT7 : MNV-G 3'Rz, but lacked the 3' hepatitis delta virus ribozyme.

The MNV 1 subgenomic RNA cDNA expression construct pT7 : MNV-SG was generated by RT-PCR amplification of RNA purified from MNV 1 CW1-infected cells, using primers IGIC21 and IGIC22 (see Supplementary Table S1, available in JGV Online). The amplified product was digested with NotI and SwaI and inserted into pTriEx1.1 (Novagen) between the NotI and MscI sites. The construct was then sequenced fully to confirm that it matched the reported CW1 passage 3 consensus sequence.

Virus recovery and characterization.
Cells were infected with poxviruses expressing T7 RNA polymerase at an m.o.i. (based on the virus titre in chick embryo fibroblasts) of 0.5–1.0 p.f.u. per cell. Each cDNA expression construct or VPg-linked viral RNA, purified as described previously (Chaudhry et al., 2006), was subsequently transfected (1 µg) by using Lipofectamine 2000 according to the manufacturer's instructions (Invitrogen). To analyse protein expression, cells were harvested 24 h post-transfection for Western blot analysis. To examine the presence of infectious norovirus, cells were harvested 24–72 h post-transfection, virus was released by two freeze–thaw cycles and the titres of virus were determined as TCID₅₀ in RAW 264.7 cells, using microscopic visualization for the appearance of cytopathic effect. In some cases, plaque morphology was also examined by plaque assay (Wobus et al., 2004). One-step growth-curve analysis was performed by infecting RAW 264.7 cells at an m.o.i. of 6.0 per cell. Samples were incubated at 37 °C and frozen at –80 °C at various times post-infection. Following two freeze–thaw cycles, the virus titre was determined by TCID₅₀ on RAW 264.7 cells.

Identification of nuclease-resistant, encapsidated MNV RNA.
To remove unencapsidated MNV RNA or excess cDNA, clarified lysates from transfected cells were treated with DNase I (10 units ml^–1), RNase A (10 units ml^–1) and RNase T1 (400 units ml^–1) at 37 °C for 2 h. Encapsidated RNA was partially purified by centrifugation through a 30 % sucrose cushion for 1 h at 55 000 r.p.m. using a Beckman SW55 Ti rotor. The viral pellet was DNase- and RNase-treated prior to extraction of the viral RNA, which used the GenElute system (Sigma). The viral RNA was detected by RT-PCR amplification using the primers 7155F and 7400R (see Supplementary Table S1, available in JGV Online), resulting in the amplification of a 258 bp product.

Sequence and RT-PCR analyses of recovered viruses.
To determine the sequence of the viruses recovered from cDNA, RAW 264.7 cells were infected with the recovered viruses at an m.o.i. of 3.0 and viral RNA was prepared 24 h post-infection by using the GenElute system (Sigma). Seven overlapping PCR products were amplified, covering the entire genome, and the sequence was determined by using a series of primers (Wobus et al., 2004). To determine the sequence of the 5' and 3' ends, 5' and 3' rapid amplification of cDNA ends (RACE) was performed by using the Advantage RACE system (Clontech). Sequence analysis and contig generation were performed by using Vector NTI (Invitrogen).

	RESULTS

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VACV infection inhibits MNV replication
Previous calicivirus reverse-genetics systems have relied on the transfection of either in vitro-transcribed, 5'-capped calicivirus genomic RNA (Chang et al., 2005; Sosnovtsev & Green, 1995) or cDNA constructs, followed by delivery of T7 RNA polymerase using a VACV recombinant (Sosnovtsev et al., 2002; Thumfart & Meyers, 2002). A recent report on rabbit hemorrhagic disease virus (RHDV) has also demonstrated that in vitro-transcribed, uncapped RNA is infectious when transfected into cells or delivered directly to the liver in vivo (Liu et al., 2006). Attempts to recover MNV by using any of these established approaches failed to produce infectious virus (data not shown). Results indicated that capped, in vitro-transcribed MNV RNA is not translated efficiently when transfected into cells (data not shown) and that VACV infection can have a detrimental effect on MNV replication (Fig. 2a). Levels of the viral RNA-dependent RNA polymerase NS7 and the minor capsid protein VP2 in cells transfected with VPg-linked RNA were reduced significantly when cells had previously been infected with a VACV expressing T7 RNA polymerase (MVA-T7) (Wyatt et al., 1995; Fig. 2a). This reduction in NS7 and VP2 resulted in a decrease of approximately 200-fold in virus yield (Fig. 2a). In contrast, prior infection of cells with an FWPV recombinant expressing T7 RNA polymerase (FPV-T7) (Britton et al., 1996) had no effect on NS7, VP2 or virus titre (Fig. 2a).

View larger version (15K): [in this window] [in a new window]   Fig. 2. Analysis of the effect of poxvirus infection on MNV replication. (a) BHK cells were mock-infected (M) or infected with either VACV (MVA-T7) or FWPV (FPV-T7) expressing T7 RNA polymerase and subsequently transfected with MNV VPg-linked RNA. Levels of the viral RNA-dependent RNA polymerase (NS7) and minor capsid protein (VP2) were analysed by Western blotting with rabbit polyclonal antisera. In parallel, the virus yield was determined and expressed as TCID50 per 35 mm dish. Transfections were carried out in triplicate; error bars represent SD. (b) BHK cells were either mock-infected (M) or infected with MVA-T7 or FPV-T7 and subsequently transfected with a cDNA construct containing the entire MNV genome under the control of a T7 RNA polymerase promoter (pT7 : MNV-G). NS7 expression levels were subsequently analysed by Western blotting.

FWPV expressing T7 RNA polymerase allows recovery of MNV
Given our observation that FPV-T7 had no deleterious effect on MNV replication, yet was able to drive efficient expression of MNV proteins, the ability of FPV-T7 to allow the recovery of genetically defined norovirus in tissue culture was examined (Fig. 3). FPV-T7-infected cells were transfected with a cDNA construct containing the full-length MNV genomic cDNA (pT7 : MNV-G; Fig. 1b), a similar construct that contained a frame-shift mutation in the viral RNA-dependent RNA polymerase NS7 (pT7 : MNV-G^FS; Fig. 1b) or a derivative of this construct in which the frame-shift mutation had subsequently been repaired (pT7 : MNV-G^FS/R). To examine the requirement for the viral capsid proteins VP1 and VP2, cells were co-transfected with either empty vector or a cDNA construct containing the MNV subgenomic RNA (pT7 : MNV-SG). Western blot analysis demonstrated that high levels of NS7 were detected in cells transfected with either VPg-linked viral RNA or pT7 : MNV-G (Fig. 3a). As predicted, a truncated NS7, referred to as NS7', was detected in cells transfected with pT7 : MNV-G^FS (Fig. 3a), whereas full-length NS7 was detected in cells that had been transfected with a construct in which the frame-shift mutation had been repaired (pT7 : MNV-G^FS/R; Fig. 3a). The viral capsid proteins VP1 and VP2 were only detected in cells transfected with the subgenomic cDNA expression construct pT7 : MNV-SG [Fig. 3(a) for VP1; data not shown for VP2].

View larger version (64K): [in this window] [in a new window]   Fig. 3. Recovery of genetically defined noroviruses in tissue culture. (a) Western blot analysis of BHK cells transfected with either purified VPg-linked MNV RNA (vRNA) or plasmids expressing the cDNA encompassing the MNV subgenomic RNA [pT7 : MNV-SG (SG)], genomic RNA [pT7 : MNV-G (G)], genomic RNA containing a frame-shift mutation in the region coding for NS7 [pT7 : MNV-GFS (GFS)] or the repaired derivative [pT7 : MNV-GFS/R (GFS/R)]. Samples where infectious virus was recovered are indicated by +. (b) RT-PCR analysis demonstrating the presence of nuclease-resistant MNV RNA in nuclease-treated supernatants. PCRs were carried out with and without the prior addition of reverse transcriptase (RT). Positive and negative controls for PCR amplification (PCR– and PCR+) contained nuclease-free water or a plasmid encoding the MNV genomic RNA, respectively. Size of molecular mass markers is indicated.

The presence of infectious virus was subsequently confirmed by the ability to passage infectivity repeatedly to RAW 264.7 murine macrophages and confirmed by Western blot analysis of infected cells (data not shown). Infectious virus was reproducibly produced only from cells that had been transfected with purified viral RNA or transfected with cDNA constructs for both the full-length genomic and subgenomic RNAs (Fig. 3a). As expected, a frame-shift mutation in NS7 prevented the recovery of infectious virus, which was subsequently recovered when the mutation was repaired (Fig. 3a).

Recovery of genetically tagged MNV
To confirm that the reverse-genetics system allowed the recovery of genetically defined noroviruses, an additional BglII restriction site was introduced into the MNV genome within the region encoding NS7. A single-nucleotide change (C to A) at position 3959 resulted in the introduction of a BglII site (Fig. 4a). Recombinant viruses were recovered from cells co-transfected with a cDNA expression construct for the viral subgenomic RNA (pT7 : MNV-SG) along with either the wild-type full-length genomic cDNA construct (pT7 : MNV-G) or an identical construct containing the additional BglII restriction site (pT7 : MNV-G/BglII). The recovered viruses, referred to as CW1-R and CW1-Bgl, were subsequently amplified in tissue culture, and RT-PCR analysis of the region encoding NS7 was performed by using primers 3734F and 4450R. BglII digestion of the 746 bp amplified products demonstrated the presence of a single BglII site in the amplicons from the parental and recombinant MNV, CW1 and CW1-R (Fig. 4b). However, an additional BglII site was present in the amplicon generated from the BglII-tagged virus, as evident by the generation of a 107 bp fragment (CW1-Bgl; Fig. 4b). Direct sequencing of the amplicons confirmed the presence of the additional BglII site (Fig. 4c). The entire sequence of the recovered viruses was determined by RT-PCR combined with 5' and 3' RACE, and no additional nucleotide changes were observed in either CW1-R or CW1-Bgl.

View larger version (36K): [in this window] [in a new window]   Fig. 4. Recovery of genetically marked MNV. (a) Schematic representation of the mutated region of the MNV genome. The additional BglII restriction site introduced in the recombinant virus CW1-Bgl is indicated by an asterisk. (b) RT-PCR amplification and subsequent digestion of the amplified region, indicating the presence of an additional BglII site in the mutated virus CW1-Bgl that is absent in the parental recombinant CW1 virus derived from cDNA (CW1-R) or tissue culture-adapted MNV (CW1). Size of molecular mass markers is indicated (in bp). (c) Sequencing chromatogram of the RT-PCR products encompassing the mutated region of CW1 and CW1-Bgl. The nucleotide change introduced in CW1-Bgl is underlined; the introduced BglII site is indicated by a black line.

View larger version (29K): [in this window] [in a new window]   Fig. 5. Growth characteristics of noroviruses recovered from cDNA. Plaque phenotype (a) and one-step growth-curve analysis (b) of wild-type MNV (CW1, ), MNV recovered entirely from cDNA (CW1-R, ) and the recombinant MNV containing the additional BglII site (CW1-Bgl, ).

	DISCUSSION

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Also worth noting is the fact that the T7 RNA polymerase in the MVA-T7 used in this study is under the control of a late (p11) poxvirus promoter (Wyatt et al., 1995), whereas that in FPV-T7 is under the control of the early/late poxvirus promoter, p7.5 (Britton et al., 1996). It is conceivable that the use of an MVA-T7 expressing T7 RNA polymerase from an early/late promoter (Sutter et al., 1995) might have proved capable of rescuing MNV. However, the observation that equivalent levels of MNV proteins were expressed from pT7 : MNV-G in cells infected by either MVA-T7 or FPV-T7 argues somewhat against this. The inhibitory effect of MVA-induced cytopathic effect on expression from VPg-linked RNA might have been countered by the use of cytosine arabinoside, which blocks MVA genome replication. Such a strategy was used successfully to rescue measles virus (Kovacs et al., 2003), but again, it would have required the use of an MVA with T7 polymerase under the control of an early or early/late promoter.

Our inability to recover MNV by transfection of in vitro-transcribed, capped or uncapped RNA is in contrast to previous reports on FCV (Sosnovtsev & Green, 1995; Thumfart & Meyers, 2002), PEC (Chang et al., 2005) and RHDV (Liu et al., 2006). It is probable that this simply reflects the poor stability of the RNA or the inability of the host-cell translation machinery to translate capped or uncapped MNV RNA efficiently. Indeed, our previous work on calicivirus translation would indicate that VPg is required for efficient translation of calicivirus RNA (Goodfellow et al., 2005; Chaudhry et al., 2006). We have also demonstrated that, despite the ability of MNV VPg to interact with eIF4E, VPg-linked MNV viral RNA is able to translate in the absence of eIF4E in vitro (Chaudhry et al., 2006). This indicates that translation initiation on MNV RNA requires a subset of initiation factors different from that required by capped host-cell mRNAs. Our unpublished data would confirm that in vitro translation of capped or uncapped MNV RNA is inefficient compared with that of VPg-linked viral RNA (data not shown).

During our study, we also examined the ability of the BSR-T7 cell line, a BHK cell line derivative that expresses T7 RNA polymerase constitutively, to allow the recovery of MNV in the absence of FWPV infection (Table 2). This cell line was chosen due to the reported success in recovery of respiratory syncytial virus (Buchholz et al., 1999) and bunyaviruses (Lowen et al., 2004), as well as a potential method of helper-free virus recovery. However, we failed to detect MNV protein expression after transfection of the BSR-T7 cell line with MNV cDNA constructs (data not shown). Protein expression and infectious virus were only detected after prior infection with FPV-T7 (data not shown). This may be due to low levels of RNA synthesis in these cells in the absence of FPV-T7 infection or, as described above, to the fact that the uncapped MNV transcripts produced in this cell line are either unstable or poorly translated. Although previous reports would suggest that between 5 and 10 % of the transcripts produced by T7 RNA polymerase in VACV-infected cells are capped (Fuerst & Moss, 1989), similar studies have not been carried out for FPV-T7. It is likely that some of the transcripts produced by using the FPV-T7 system are capped by the fowlpox capping enzymes; however, future studies would be required to confirm this.

Given the previously reported role of interferon in controlling calicivirus replication (Karst et al., 2003; Chang et al., 2004; Wobus et al., 2004), we examined the recovery of virus by using the reverse-genetics system from cell lines defective for various aspects of the interferon response (Vero and Huh 7.5 cells). However, the yield of virus from these cell lines was no greater than that obtained from cells in which the interferon system was intact (Table 2). In fact, the Vero cell line, defective for interferon synthesis (Emeny & Morgan, 1979), failed to recover any infectious virus and appeared to replicate MNV to only low levels. Further studies also demonstrated that expressing the V protein from simian virus 5, which is known to lead to the degradation of STAT-1 (Andrejeva et al., 2002), had no stimulatory effect on MNV recovery in 293 cells (data not shown). Hence, our data would indicate that the interferon system plays no role in the restriction of virus recovery using the reverse-genetics system, although further studies are warranted.

Our results would also suggest that the sequence of the 3'-terminal nucleotide of the MNV genome is critical for efficient recovery, as constructs containing an incorrect 3'-terminal nucleotide required the co-expression of the MNV subgenomic RNA for recovery (Fig. 3a; Table 1). Interestingly, viruses recovered by using the genomic RNA construct that contained an incorrect 3'-terminal nucleotide appeared to correct the 3'-terminal nucleotide to match that present in all previously sequenced MNV strains (thymidine; data not shown). It is possible that the repair of the 3'-end defect was the result of low-frequency recombination between the genomic and subgenomic RNAs; however, further studies would be required to confirm this. The inclusion of a hepatitis delta ribozyme at the 3' end of the viral genome was found to increase virus yield and resulted in maximal virus production 24 h post-transfection (Table 2), possibly indicating that a free 3' end is required for efficient virus replication.

Seroprevalence studies have highlighted that, as well as functioning as a model for the human noroviruses, MNV is a significant pathogen in its own right, with 22 % of mouse colonies in the USA and Canada found to be seropositive (Hsu et al., 2005). Recent studies have also highlighted the fact that numerous strains appear to circulate, which can differ markedly in their ability to replicate and cause disease in the host (Hsu et al., 2006; Mumphrey et al., 2007). As more strains are identified, by combining sequence data, the mouse model and the reverse-genetics system described herein, it will now be possible to correlate sequence variation with differences in norovirus pathogenicity. Undoubtedly, such studies will facilitate the identification of viral and host-cell factors required for norovirus pathogenesis and will aid our ability to control members of this economically important family of viruses.

	ACKNOWLEDGEMENTS

 
The authors would like to thank Herbert Virgin IV, Christiane Wobus, Larissa Thackray and Ioannis Karakasiliotis for supplying reagents and helpful comments during the course of the work. This work was supported by a Wellcome Trust career development fellowship to I. G. G., as well as funding from the BBSRC to both I. G. G. and M. A. S.

	REFERENCES

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

 
Andrejeva, J., Young, D. F., Goodbourn, S. & Randall, R. E. (2002). Degradation of STAT1 and STAT2 by the V proteins of simian virus 5 and human parainfluenza virus type 2, respectively: consequences for virus replication in the presence of alpha/beta and gamma interferons. J Virol 76, 2159–2167.[Abstract/Free Full Text]

Asanaka, M., Atmar, R. L., Ruvolo, V., Crawford, S. E., Neill, F. H. & Estes, M. K. (2005). Replication and packaging of Norwalk virus RNA in cultured mammalian cells. Proc Natl Acad Sci U S A 102, 10327–10332.[Abstract/Free Full Text]

Baron, M. D. & Barrett, T. (1997). Rescue of rinderpest virus from cloned cDNA. J Virol 71, 1265–1271.[Abstract]

Boot, H. J., ter Huurne, A. A., Peeters, B. P. & Gielkens, A. L. (1999). Efficient rescue of infectious bursal disease virus from cloned cDNA: evidence for involvement of the 3'-terminal sequence in genome replication. Virology 265, 330–341.[CrossRef][Medline]

Britton, P., Green, P., Kottier, S., Mawditt, K. L., Penzes, Z., Cavanagh, D. & Skinner, M. A. (1996). Expression of bacteriophage T7 RNA polymerase in avian and mammalian cells by a recombinant fowlpox virus. J Gen Virol 77, 963–967.[Abstract/Free Full Text]

Buchholz, U. J., Finke, S. & Conzelmann, K.-K. (1999). Generation of bovine respiratory syncytial virus (BRSV) from cDNA: BRSV NS2 is not essential for virus replication in tissue culture, and the human RSV leader region acts as a functional BRSV genome promoter. J Virol 73, 251–259.[Abstract/Free Full Text]

Casais, R., Thiel, V., Siddell, S. G., Cavanagh, D. & Britton, P. (2001). Reverse genetics system for the avian coronavirus infectious bronchitis virus. J Virol 75, 12359–12369.[Abstract/Free Full Text]

Chang, K. O., Kim, Y., Green, K. Y. & Saif, L. J. (2002). Cell-culture propagation of porcine enteric calicivirus mediated by intestinal contents is dependent on the cyclic AMP signaling pathway. Virology 304, 302–310.[CrossRef][Medline]

Chang, K. O., Sosnovtsev, S. V., Belliot, G., Kim, Y., Saif, L. J. & Green, K. Y. (2004). Bile acids are essential for porcine enteric calicivirus replication in association with down-regulation of signal transducer and activator of transcription 1. Proc Natl Acad Sci U S A 101, 8733–8738.[Abstract/Free Full Text]

Chang, K.-O., Sosnovtsev, S. S., Belliot, G., Wang, Q., Saif, L. J. & Green, K. Y. (2005). Reverse genetics system for porcine enteric calicivirus, a prototype sapovirus in the Caliciviridae. J Virol 79, 1409–1416.[Abstract/Free Full Text]

Chang, K.-O., Sosnovtsev, S. V., Belliot, G., King, A. D. & Green, K. Y. (2006). Stable expression of a Norwalk virus RNA replicon in a human hepatoma cell line. Virology 353, 463–473.[CrossRef][Medline]

Chaudhry, Y., Nayak, A., Bordeleau, M.-E., Tanaka, J., Pelletier, J., Belsham, G. J., Roberts, L. O. & Goodfellow, I. G. (2006). Caliciviruses differ in their functional requirements for eIF4F components. J Biol Chem 281, 25315–25325.[Abstract/Free Full Text]

Clarke, D. K., Sidhu, M. S., Johnson, J. E. & Udem, S. A. (2000). Rescue of mumps virus from cDNA. J Virol 74, 4831–4838.[Abstract/Free Full Text]

Das, S. C., Baron, M. D., Skinner, M. A. & Barrett, T. (2000). Improved technique for transient expression and negative strand virus rescue using fowlpox T7 recombinant virus in mammalian cells. J Virol Methods 89, 119–127.[CrossRef][Medline]

Emeny, J. M. & Morgan, M. J. (1979). Regulation of the interferon system: evidence that Vero cells have a genetic defect in interferon production. J Gen Virol 43, 247–252.[Abstract/Free Full Text]

Fuerst, T. R. & Moss, B. (1989). Structure and stability of mRNA synthesized by vaccinia virus-encoded bacteriophage T7 RNA polymerase in mammalian cells. Importance of the 5' untranslated leader. J Mol Biol 206, 333–348.[CrossRef][Medline]

Fuerst, T. R., Niles, E. G., Studier, F. W. & Moss, B. (1986). Eukaryotic transient expression system based on recombinant vaccinia virus that synthesizes bacteriophage T7 RNA polymerase. Proc Natl Acad Sci U S A 83, 8122–8126.[Abstract/Free Full Text]

Gassen, U., Collins, F. M., Duprex, W. P. & Rima, B. K. (2000). Establishment of a rescue system for canine distemper virus. J Virol 74, 10737–10744.[Abstract/Free Full Text]

Goodfellow, I., Chaudhry, Y., Gioldasi, I., Gerondopoulos, A., Natoni, A., Labrie, L., Lailiberte, J. & Roberts, L. (2005). Calicivirus translation initiation requires an interaction between VPg and eIF4E. EMBO Rep 6, 968–972.[CrossRef][Medline]

Hsu, C. C., Wobus, C. E., Steffen, E. K., Riley, L. K. & Livingston, R. S. (2005). Development of a microsphere-based serologic multiplexed fluorescent immunoassay and a reverse transcriptase PCR assay to detect murine norovirus 1 infection in mice. Clin Diagn Lab Immunol 12, 1145–1151.[CrossRef][Medline]

Hsu, C. C., Riley, L. K., Wills, H. M. & Livingston, R. S. (2006). Persistent infection with and serologic cross-reactivity of three novel murine noroviruses. Comp Med 56, 247–251.[Medline]

Karst, S. M., Wobus, C. E., Lay, M., Davidson, J. & Virgin, H. W., IV (2003). STAT1-dependent innate immunity to a Norwalk-like virus. Science 299, 1575–1578.[Abstract/Free Full Text]

Katayama, K., Hansman, G. S., Oka, T., Ogawa, S. & Takeda, N. (2006). Investigation of norovirus replication in a human cell line. Arch Virol 151, 1291[CrossRef][Medline]

Kovacs, G. R., Parks, C. L., Vasilakis, N. & Udem, S. A. (2003). Enhanced genetic rescue of negative-strand RNA viruses: use of an MVA-T7 RNA polymerase vector and DNA replication inhibitors. J Virol Methods 111, 29–36.[CrossRef][Medline]

Leyrer, S., Neubert, W. J. & Sedlmeier, R. (1998). Rapid and efficient recovery of Sendai virus from cDNA: factors influencing recombinant virus rescue. J Virol Methods 75, 47–58.[CrossRef][Medline]

Liu, G., Zhang, Y., Ni, Z., Yun, T., Sheng, Z., Liang, H., Hua, J., Li, S., Du, Q. & Chen, J. (2006). Recovery of infectious rabbit hemorrhagic disease virus from rabbits after direct inoculation with in vitro-transcribed RNA. J Virol 80, 6597–6602.[Abstract/Free Full Text]

Lopman, B. A., Reacher, M. H., Van Duijnhoven, Y., Hanon, F. X., Brown, D. & Koopmans, M. (2003). Viral gastroenteritis outbreaks in Europe, 1995–2000. Emerg Infect Dis 9, 90–96.[Medline]

Lowen, A. C., Noonan, C., McLees, A. & Elliott, R. M. (2004). Efficient bunyavirus rescue from cloned cDNA. Virology 330, 493[CrossRef][Medline]

Mumphrey, S. M., Changotra, H., Moore, T. N., Heimann-Nichols, E. R., Wobus, C. E., Reilly, M. J., Moghadamfalahi, M., Shukla, D. & Karst, S. M. (2007). Murine norovirus 1 infection is associated with histopathological changes in immunocompetent hosts but clinical disease is prevented by STAT1-dependent interferon responses. J Virol 81, 3251–3263.[Abstract/Free Full Text]

Peeters, B. P., de Leeuw, O. S., Koch, G. & Gielkens, A. L. (1999). Rescue of Newcastle disease virus from cloned cDNA: evidence that cleavability of the fusion protein is a major determinant for virulence. J Virol 73, 5001–5009.[Abstract/Free Full Text]

Schneider, H., Spielhofer, P., Kaelin, K., Dotsch, C., Radecke, F., Sutter, G. & Billeter, M. A. (1997). Rescue of measles virus using a replication-deficient vaccinia-T7 vector. J Virol Methods 64, 57–64.[CrossRef][Medline]

Sosnovtsev, S. & Green, K. Y. (1995). RNA transcripts derived from a cloned full-length copy of the feline calicivirus genome do not require VPg for infectivity. Virology 210, 383–390.[CrossRef][Medline]

Sosnovtsev, S. V., Garfield, M. & Green, K. Y. (2002). Processing map and essential cleavage sites of the nonstructural polyprotein encoded by ORF1 of the feline calicivirus genome. J Virol 76, 7060–7072.[Abstract/Free Full Text]

Sosnovtsev, S. V., Belliot, G., Chang, K.-O. K., Prikhodko, V. G., Thackray, L. B., Wobus, C. E., Karst, S. M., Virgin, H. W. & Green, K. Y. (2006). Cleavage map and proteolytic processing of the murine norovirus nonstructural polyprotein in infected cells. J Virol 80, 7816–7831.[Abstract/Free Full Text]

Sumpter, R., Jr, Loo, Y.-M., Foy, E., Li, K., Yoneyama, M., Fujita, T., Lemon, S. M. & Gale, M., Jr (2005). Regulating intracellular antiviral defense and permissiveness to hepatitis C virus RNA replication through a cellular RNA helicase, RIG-I. J Virol 79, 2689–2699.[Abstract/Free Full Text]

Sutter, G., Ohlmann, M. & Erfle, V. (1995). Non-replicating vaccinia vector efficiently expresses bacteriophage T7 RNA polymerase. FEBS Lett 371, 9–12.[CrossRef][Medline]

Thumfart, J. O. & Meyers, G. (2002). Feline calicivirus: recovery of wild-type and recombinant viruses after transfection of cRNA or cDNA constructs. J Virol 76, 6398–6407.[Abstract/Free Full Text]

Walker, S. C., Avis, J. M. & Conn, G. L. (2003). General plasmids for producing RNA in vitro transcripts with homogeneous ends. Nucleic Acids Res 31, e82[Abstract/Free Full Text]

Wobus, C. E., Karst, S. M., Thackray, L. B., Chang, K. O., Sosnovtsev, S. V., Belliot, G., Krug, A., Mackenzie, J. M., Green, K. Y. & Virgin, H. W. (2004). Replication of norovirus in cell culture reveals a tropism for dendritic cells and macrophages. PLoS Biol 2, e432[CrossRef][Medline]

Wyatt, L. S., Moss, B. & Rozenblatt, S. (1995). Replication-deficient vaccinia virus encoding bacteriophage T7 RNA polymerase for transient gene expression in mammalian cells. Virology 210, 202–205.[CrossRef][Medline]

Yunus, A. S., Khattar, S. K., Collins, P. L. & Samal, S. K. (2001). Rescue of bovine respiratory syncytial virus from cloned cDNA: entire genome sequence of BRSV strain A51908. Virus Genes 23, 157–164.[CrossRef][Medline]

Received 21 February 2007; accepted 19 April 2007.

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