Effect of Intragenic Rearrangement and Changes in the 3' Consensus Sequence on NSP1 Expression and Rotavirus Replication

doi:10.1128/JVI.75.5.2076-2086.2001

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Journal of Virology, March 2001, p. 2076-2086, Vol. 75, No. 5
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.5.2076-2086.2001

Effect of Intragenic Rearrangement and Changes in the 3' Consensus Sequence on NSP1 Expression and Rotavirus Replication

John T. Patton,¹^,^* Zenobia Taraporewala,¹ Dayue Chen,¹ Vladimir Chizhikov,¹ Melinda Jones,¹ Azza Elhelu,¹ Megan Collins,¹ Karen Kearney,¹ Mariam Wagner,¹ Yasutaka Hoshino,¹ and Vera Gouvea²

Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, Bethesda, Maryland,¹ and Department of Virology, Institute of Microbiology, Universidade Federal do Rio de Janeiro, Rio de Janeiro, RJ 21941-590, Brazil²

Received 24 August 2000/Accepted 30 November 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The nonpolyadenylated mRNAs of rotavirus are templates for the synthesis of protein and the segmented double-stranded RNA(dsRNA) genome. During serial passage of simian SA11 rotavirusesin cell culture, two variants emerged with gene 5 dsRNAs containinglarge (1.1 and 0.5 kb) sequence duplications within the open readingframe (ORF) for NSP1. Due to the sequence rearrangements, bothvariants encoded only C-truncated forms of NSP1. Comparison ofthese and other variants encoding defective NSP1 with their correspondingwild-type viruses indicated that the inability to encode authenticNSP1 results in a small-plaque phenotype. Thus, although nonessential,NSP1 probably plays an active role in rotavirus replication incell culture. In determining the sequences of the gene 5 dsRNAsof the SA11 variants and wild-type viruses, it was unexpectedlyfound that their 3' termini ended with 5'-UGAACC-3' instead ofthe 3' consensus sequence 5'-UGACC-3', which is present on themRNAs of nearly all other group A rotaviruses. Cell-free assaysindicated that the A insertion into the 3' consensus sequenceinterfered with its ability to promote dsRNA synthesis and tofunction as a translation enhancer. The results provide evidencethat the 3' consensus sequence of the gene 5 dsRNAs of SA11 rotaviruseshas undergone a mutation causing it to operate suboptimally inRNA replication and in the expression of NSP1 during the viruslife cycle. Indeed, just as rotavirus variants which encode defectiveNSP1 appear to have a selective advantage over those encodingwild-type NSP1 in cell culture, it may be that the atypical 3'end of SA11 gene 5 has been selected for because it promotes theexpression of lower levels of NSP1 than the 3' consensussequence.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Rotavirus virions are icosahedral particles consisting of three layers of protein and containing 11 segments of double-strandedRNA (dsRNA) (8). The innermost protein layer has a T=2 arrangementand is formed by the core lattice protein VP2 (reviewed in reference29). Associated with the interior side of each of the 12 pentamersof the VP2 lattice is believed to be one copy each of the viralRNA-dependent RNA polymerase (RdRP) VP1 and the mRNA-capping enzymeVP3 (19, 20). Based on structural studies of rotaviruses andother members of the family Reoviridae (29), it is thought thateach genome segment exists as a tightly wound spiral around oneof the 12 RdRP-capping complexes of the VP2 lattice (9). Collectively,the VP2 lattice, the RdRP-capping complexes, and the dsRNA genomemake up the core of the virion. Double-layered particles consistingof cores surrounded by the intermediate protein VP6 have transcriptaseactivity and are responsible for the synthesis of the 11 viralmRNAs (1, 37). The dsRNA genome probably exists as a liquidcrystal within the core and, in this form, has the fluidity necessaryfor the dsRNA segments to slide through the anchored RdRP-cappingenzyme complex during transcription (9). Nascent transcriptsproduced by the viral RdRP are extruded through channels locatedat the vertices of double-layered particles (18).

Translation of the viral mRNAs yields six structural (VP1 to VP4, VP6, and VP7) and six nonstructural (NSP1 to NSP6) proteins(8). In the viral life cycle, the mRNAs are also used by theviral RdRP as templates for the synthesis of minus-strand RNAs,resulting in the formation of dsRNAs (3, 29). The rotavirusmRNAs are unique in that, although they possess methylated 5'caps, they lack 3' poly(A) tails (15, 23). Except for shortsequences at their 5' and 3' termini, the 11 viral mRNAs exhibitno sequence similarity. The 3'-terminal sequence of the mRNAsof the group A rotaviruses has consistently been reported to be5'-UGACC-3' (8). Several studies have illustrated the importanceof this 3' consensus sequence in the viral life cycle. In particular,template-dependent cell-free replication systems have shown thatthe 3' consensus sequence contains a cis-acting signal that isessential for the viral mRNA to function efficiently as a templatefor minus-strand synthesis (31, 42). Moreover, the last fournucleotides of the conserved sequence form a signal (3' translationenhancer) that enhances translation of the viral mRNAs (4).The upregulation of gene expression is mediated by NSP3, a proteinwhich is believed to cause circularization of viral mRNAs in polysomesby simultaneously binding to the 3' consensus sequence and tothe cap binding protein eIF4G (34, 35, 41).

Rotaviruses with atypical genome segments have been recovered from animals and immunocompromised children and have been generatedby serial passage of the virus at high multiplicity of infection(MOI) in cell culture (7, 13, 40). In most cases, molecularanalysis has shown that the atypical genome segments contain ahead-to-tail duplication of sequences within the dsRNA (5,14, 24, 32, 36). Such sequence rearrangements have beenidentified for segments 5 to 7, 10, and 11 (6). So far, thesequence duplications that have been described for segments 6,7, 10, and 11 begin after the open reading frame (ORF) and, asa result, the rearrangement does not affect the ability of theRNAs to encode full-length proteins. In contrast, most of thesequence duplications described for segment 5 begin within theORF and alter the coding capacity of the gene such that it nolonger encodes wild-type NSP1 (10, 40). Other atypical genomesegments 5 have been identified which, instead of containing duplicatedsequences, contain sequence deletions or nonsense mutations withinthe ORF that also prevent the gene from encoding wild-type NSP1(38, 40). The fact that rotaviruses can replicate in cellculture, even when unable to produce wild-type NSP1, has led tothe suggestion that the protein is nonessential. The role of NSP1in the viral life cycle is uncertain, but the protein is knownto bind RNA and to be associated with the cytoskeleton fractionof infected cells (11).

In this study, we have characterized two variants of simian rotavirus SA11 whose gene 5 dsRNAs contain rearrangements stemmingfrom duplication of sequences located within the NSP1 ORF. Therearrangements altered the ORFs such that they encoded C-truncatedNSP1. Like other NSP1-defective isolates, the two variants displayeda small-plaque phenotype, suggesting that NSP1 contributes tothe viral life cycle even in cell culture. Remarkably, sequencingalso revealed that the 3' termini of the segment 5 dsRNAs of thevariants and of wild-type SA11 were atypical (UGAACC) in thatthey contained an A insertion relative to the expected 3' consensussequence (UGACC). The fact that the wild-type SA11 viruses grewto high titer and produced NSP1 demonstrated that the 3' consensussequence is not required for genome packaging, RNA replication,or viral gene expression. However, in vitro assays indicated thatthe A insertion altered the 3' consensus sequence such that itoperated suboptimally in replication and geneexpression.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Isolation of rotavirus variants 30-1A and 5S. The simian SA11 strain SA11-FEM (26) was received from G. W. Gary (Centers for Disease Control and Prevention, Atlanta,Ga.), and the SA11-4F strain (22, 33) was received from R.L. Ward (Children's Hospital Medical Center, Cleveland, Ohio),who had obtained the strain from M. K. Estes (Baylor College ofMedicine, Houston, Tex.). Both of these SA11 strains carry a bovinerotavirus-like VP4 gene, and both were originally provided byH. H. Marlherbe (21). The simian SA11 strains of rotavirus SA11-FEMand SA11-4F were serially passaged without dilution in MA104 cells.The gene 5 variant 30-1A and its wild-type correlate 30-19 wereisolated by triple-plaque purification from the passage 30 lysateof SA11-FEM-infected cells, and the gene 5 variant 5S was obtainedby limiting dilution from the passage 26 lysate of SA11-4F-infectedcells. Viruses were propagated in the presence of 0.5 µg of trypsinper ml, and titers were determined by plaque assay on MA104 cells(30). The diameter of plaques was measured 5 days post-infection(p.i.).

Genomic dsRNAs were purified from rotavirus particles by phenol-chloroform extraction and ethanol precipitation. The genotypesof the viruses were examined by electrophoresis of purified dsRNAon 12% polyacrylamide gels containing sodium dodecyl sulfate (SDS-12%PAGE), followed by staining with ethidium bromide (30).

cDNA cloning and sequencing of gene 5 dsRNAs. To prepare full-length gene 5 cDNAs, purified dsRNAs were denatured by resuspension in water and heating to 95°C for 5 minor by resuspension in 90% dimethyl sulfoxide and heating to 65°Cfor 10 min. First-strand cDNAs were synthesized by incubatingthe denatured RNA with Superscript II reverse transcriptase (LifeTechnologies) and the primers 5'-ggcttttttttgaaaagtcttgtgttagcc-3'and 5'-ggttcacagtattttgccagctaggcgc-3'. The cDNAs were amplifiedby PCR using Elongase DNA polymerase (Life Technologies) and thesame primers. PCR products of the appropriate size were gel purifiedand ligated into the vector pT7Blue (Novagen). Following transformationof Escherichia coli DH5 $alpha$ , bacteria containing the appropriateplasmids (pT7-gene 5) were identified based on antibiotic resistance,plasmid size, and restriction enzyme digestion. Plasmids containingfull-length gene 5 cDNA inserts were purified with Concert maxiprepkits (Life Technologies). Due to the presence of duplicated sequencesin the rearranged gene 5 cDNAs, subclones were prepared that containedfragments of the gene 5 cDNAs of 30-1A and 5S pT7-gene 5. Thesubclones were generated by digesting 30-1A and 5S pT7-gene 5with EcoRV and with EcoRI, EcoRV, or EcoRV and PstI, respectively,and ligating the gene 5-specific fragments into plasmid SP72 orSP65(Promega).

Sequences of the 5' and 3' termini of the gene 5 dsRNAs were determined from cDNA clones obtained by rapid amplification ofcDNA 5' ends (5' RACE system, version 2.0; Life Technologies).Terminal cDNAs were prepared by incubating reaction mixtures containing20 mM Tris-HCl (pH 8.4), 50 mM KCl, 2.5 mM MgCl₂, 10 mM dithiothreitol,the four deoxynucleoside triphosphates at 400 µM each, 0.5 µgof denatured dsRNA, the appropriate primer at 100 nM, and 200U of Superscript II reverse transcriptase for 50 min at 45°C.The primers used to generate the gene 5 plus-strand cDNAs of 30-19and 30-1A and of 4F and 5S were 5'-gcgcactttgaatgtagatagc-3' and5'-gggagcagcaaatgattatacc-3', respectively. The primers used togenerate the gene 5 minus-strand cDNAs of 30-19 and 30-1A andof 4F and 5S were 5'-attttctcatcaggaactgg-3' and 5'-cacatggatcaaacaattgaag-3',respectively. The cDNAs were tailed by incubation with 10 U ofterminal deoxynucleotidyl transferase (Life Technologies) and200 µM dATP. Subsequently, the tailed cDNAs were amplified byPCR using the poly(T)-containing anchor primer 5'-cggctcgagtttttttttttttttttttt-3'(XhoI site underlined) and gene 5-specific primers (5'-taaggatccaatgtcaataaaatcaacggagg-3'and 5'-taaggatccgcaaatgaggttcattgtcaagg-3' for the plus-strandcDNAs of 30-19 and 30-1A and of 4F and 5S, respectively, or 5'-ctgggatccaaatagaatttgcaccaatgttgc-3'and 5'-atcggatcccgccagtgtcagttgaaggta-3' for the minus-strandcDNAs of 30-19 and 30-1A and of 4F and 5S, respectively (BamHIsites underlined). The cDNA products were purified, digested withXhoI and BamHI, and ligated into the XhoI/BamHI sites ofpUC19.

Gene 5 sequences were obtained either with an ABI Prism 310 Genetic Analyzer (PE Applied Biosystems) or with a Sequenase kit(Amersham Life Science) and suitable oligonucleotideprimers.

Viral protein synthesis in infected cells. Monolayers of MA104 cells were mock infected or infected with the 30-19, 30-1A, 4F, or 5S strain of rotavirus. Beginning at1 h p.i., the cells were maintained in 80% Met- and Cys-free minimalessential medium containing 5 µg of actinomycin D per ml, andat 3 h p.i., ³⁵S-Express (1,175 mCi per mmol; NEN) was added to the medium toa final concentration of 17 µCi/ml. At 8 h p.i., the monolayerswere rinsed twice with cold, dilute reticulocyte standard buffer(RSB; 3 mM Tris-HCl [pH 8.5], 0.5 mM MgCl₂, 3 mM NaCl), and thenthe cells were scraped into dilute RSB containing 1% Triton X-100.After gentle mixing, nuclei and the cytoskeleton fraction werepelleted from the lysates by centrifugation at 3,200 × g for 2min. The pellets were resuspended in dilute RSB and, along withthe supernatant (cytosol), stored at $-$ 70°C. Proteins in the pelletsand supernatants were analyzed by SDS-10% PAGE andautoradiography.

For Western blot analysis, proteins in the soluble fraction were resolved by SDS-10% PAGE (10% NuGels; In Vitrogen) and thenelectroblotted onto a nitrocellulose sheet. The blot was blockedby soaking for 1 h in phosphate-buffered saline containing 5%skim milk. Subsequently, the blot was incubated overnight witha 1:1,000 dilution of rabbit anti-SA11 NSP1 C19 serum (11).Alkaline phosphatase-conjugated goat anti-rabbit antibody wasused as the secondary antibody at a dilution of 1:5,000. The blotswere developed with 5-bromo-4-chloro-3-indolylphosphate p-toluidinesalt and nitroblue tetrazolium chloride (LifeTechnologies).

Open-core replicase assays. Open cores were prepared from DS1 × RRV virions and treated with micrococcal nuclease to remove endogenous dsRNA (2, 30).Reaction mixtures contained 50 mM Tris-HCl (pH 7.2), 5 mM MgCl₂,5 mM dithiothreitol, 20 U of RNasin (Promega), the four deoxynucleosidetriphosphates at 200 µM each, 10 µCi of [ $alpha$ -³²P]UTP, and the indicated amount of plus-strand template RNA andopen cores. The reaction mixtures were incubated at 32°C for 2h, and the ³²P-labeled dsRNA products were resolved by SDS-12% PAGE and detectedby autoradiography. A PhosphorImager was used to quantify theamount of ³²P-labeleddsRNA.

Preparation of gene 5 mRNAs. To generate first-strand gene 5 cDNAs, SA11-4F dsRNAs were denatured by heating to 100°C for 2 min and incubated with SuperscriptII reverse transcriptase, the plus-sense primer 5'-agctctagaccgcGGCTTTTTTTTGAAAAGTCTTGTG-3',and the minus-sense primer 5'-agctctagaccgcGGTTCACAGTATTTTGCCAGC-3'(XhoI sites are underlined, and viral sequences are in uppercase).The cDNAs were then amplified by PCR using the same primers andpfu DNA polymerase (Stratagene). Afterwards, the PCR product wasdigested with XbaI and ligated into the XbaI site of the plasmidpUC19, producing the construct pUC4F5. Templates for the synthesisof SA11 gene 5 mRNAs containing the 3'-terminal sequences UGACCand UGAACC were generated by PCR. The amplification mixtures includedpfu DNA polymerase, the plus-sense primer 5'-cgcggatcctaatacgactcactataGGTTTTTTTTGAAAAGTCTTG-3'(T7 promoter is underlined), and the minus-sense primer 5'-GGTCACAGTATTTTGCCAGC-3'(UGACC)or 5'-GGTTCACAGTATTTTGCCAGC-3' (UGAACC). The mixtures also includedthe gene 5 cDNA insert released from pUC4F5 by digestion withXbaI. The PCR products were sequenced to ensure that they containedthe desired terminal sequences. Transcripts were made from thePCR templates with an Ambion MEGAscript T7 transcription kit accordingto the protocol of themanufacturer.

Construction of the NSP3 expression vector. Purified SA11 dsRNAs were denatured by resuspension in 90% dimethyl sulfoxide and heating to 95°C for 2 min. The NSP3 ORFin genome segment 7 was amplified from the denatured dsRNAs usingthe Titan One Tube Reverse Transcriptase-PCR System (BoehringerMannheim), the plus-sense primer 5'-gcttttcagatcttgATGCTCAAGATGGAGTCT-3',and the minus-sense primer 5'-gtatttgatagatctACATGTATCAAAATGGTT-3'(BglII sites are underlined, and viral sequences are in uppercase).The amplified product was gel purified, digested with BglII, andligated into isopropyl- $beta$ -D-thiogalactopyranoside (IPTG)-inducibleexpression vector pQE32 (Qiagen), which had been digested withBamHI and dephosphorylated with alkaline phosphatase (Life Technologies).Following transformation into E. coli DH5 $alpha$ , bacteria with theappropriate plasmid (pQE32g7) were identified based on antibioticresistance, plasmid size, and restriction enzyme digestion. Theexpected sequence of pQE32g7 was confirmed by automated sequencing.The plasmid pQE32g7 was then electroporated into E. coli M15 carryingthe pREP4 repressor plasmid. In pQE32g7, the NSP3 ORF is situateddownstream of sequential codons for Arg, His, Ser, and six Hisresidues.

Expression and purification of rNSP3. E. coli M15 (pREP4) containing pQE32g7 was grown to an A₆₀₀ of 0.5 in Terrific Broth (Quality Biologics), and the expressionof NSP3 was induced by adding IPTG to a final concentration of1 mM. After incubation for 4 h at 37°C, the bacteria were recoveredby centrifugation at 4,000 × g for 10 min and lysed by resuspensionin buffer containing 0.5 mM NaH₂PO₄ (pH 8), 300 mM NaCl, 5 mMimidazole, 1% Triton X-100, and 1 mg each of lysozyme, aprotinin,and leupeptin per ml. The lysate was sonicated and centrifugedat 10,000 × g for 30 min. Recombinant NSP3 (rNSP3) was purifiedfrom the pellet according to the protocol of Piron et al. (34).Briefly, the pellet was washed in 20 mM Tris-HCl (pH 8)-500 mMNaCl-5 mM imidazole and then solubilized overnight in the samebuffer containing 8 M urea. rNSP3 was purified from the solubilizedproteins with a Ni-nitrilotriacetic acid agarose column (Qiagen)and eluted with solubilization buffer, pH 4.5, containing 8 Murea. The NSP3 sample was then renatured by dialysis against 50mM Tris-HCl (pH 8.0)-150 mM NaCl-10% glycerol-0.5 mM oxidizedglutathione-5 mM reduced glutathione for 18 h at 4°C. The renaturedrNSP3 was dialyzed against low-salt buffer (2 mM Tris-HCl [pH7.2], 0.5 mM EDTA, 0.5 mM dithiothreitol) for 48 h at 4°C. Theconcentration of the purified protein was determined by Bradfordassay using bovine serum albumin as the protein standard and bycomparison with known amounts of bovine serum albumin coelectrophoresedon SDS-polyacrylamide gels and stained with Coomassie brilliantblue R-250.

Preparation of RNA probes. The DNA templates for synthesis of the ³²P-labeled RNA probes, v40-GACC and v40-GAACC, were generated by amplification withthe Expand High Fidelity PCR System (Boehringer Mannheim). Theamplification reaction mixtures contained the plasmid SP72-v40(2), the plus-sense primer 5'-taatacgactcactataG-3', and theminus-sense primer 5'-GGTCACATAAGCGCTTTC-3' or 5'-GGTTCACATAAGCGCTTTC-3'(T7 promoter is underlined, and viral sequences are in uppercase).SP72-v40 contains a sequence corresponding to the last 40 nucleotides(nt) of the SA11 gene 8 mRNA positioned downstream of the promoterfor T7 RNA polymerase. The template for the synthesis of v40 $Delta$ 3'-11was made by digesting SP72-v40 with Eco47III, which cleaves thegene 8-specific sequence in the vector 11 residues upstream fromits 3' end. The ³²P-labeled probes were made by runoff transcription using the AmbionMEGAshortscript kit according to the protocol of the manufacturer,except that the concentration of unlabeled UTP was reduced byone-fourth and 50 µCi of [ $alpha$ -³²P]UTP was included per 20 µl of reaction mixture. After runofftranscription, the RNA products were purified by phenol-chloroformextraction and isopropanol precipitation. The ³²P-labeled RNA probes were purified by electrophoresis and elutionfrom 8% polyacrylamide gels containing 7 M urea (28). RNA concentrationswere calculated from optical densities at 260nm.

The sequence of the 72-nt v40-GACC RNA was 5'-GGGAGACCGGCAGAU C U GA UAUCAU C GAU GAAU U GA U G A U G G C U U A G C A A G A A U A G A AAGCGCUUAUGUGACC-3'(2). The underlined portion of the sequence represents the3'-terminal 40 nt of the SA11 gene 8 mRNA. Except for ending withGAACC instead of GACC, the sequence of the 73-nt v40-GAACC RNAwas the same as that of the v40-GACC RNA. Although otherwise identical,the v40 $Delta$ 3'-11 RNA lacks the last 11 nt of the v40-GACCRNA.

Gel shift assays. The procedure used for analysis of rNSP3-RNA interactions by gel shift assay was similar to that described earlier (39).One pmol (~24 ng) of the ³²P-labeled RNA probe v40-GACC, v40-GAACC, or v40 $Delta$ 3'-11 was incubatedwith 5 pmol of rNSP3 in low-salt buffer in a final volume of 10µl for 30 min at room temperature. The reaction mixtures wereanalyzed by electrophoresis for 2.5 h at 175 V on nondenaturing8% polyacrylamide gels containing 50 mM Tris-HCl and 50 mM glycine(pH 8.8). Protein-probe complexes were detected on the gel byautoradiography, and the intensities of the radiolabeled bandswere measured with a PhosphorImager. The percent binding activitiesof rNSP3 for probes v40-GACC and v40-GAACC were calculated bydividing the intensity value obtained for the shifted probe withthe combined intensity values obtained for the free probe andshifted probe and then multiplying the result by100.

Preparation of g6-Fluc chimeric RNAs. The plasmid pVec2.0g6-Fluc contains the ORF for firefly luciferase situated between the 5' and 3' untranslated regions (UTRs)of the SA11 gene 6 RNA (4). The T7 transcription templatesused to produce the gene 6 analog RNAs g6-Fluc-UGACC, g6-Fluc-UGAACC,glo/g6-Fluc-UGACC, and glo/g6-Fluc-UGAACC were synthesized withthe High Fidelity PCR System (Roche Molecular Biochemicals). Thereaction mixtures contained pVec2.0g6-Fluc, the plus-sense primer5'-cccaggtaccctaatacgactcactataGGCTTTTAAACGAAGTCTTCACCATG-3' (gene6 5' UTR) or 5'-cccaggtaccctaatacgactcactatagacacttgcttctgacacacaccATGGAAGACGCCAAAAACATAAAG-3'( $beta$ -globin 5' UTR), and the minus-sense primer 5'-GGTCACATCCTCTCACTATACCATC-3'(gene 6 3' UTR, UGACC) or 5'-GGTTCACATCCTCTCACTATACCATC-3' (gene6 3' UTR, GAACC). In the primers, the T7 promoters are underlinedand the viral sequences are in uppercase. Capped mRNAs were generatedfrom the PCR products using the Ambion mMESSAGE transcriptionsystem. The quality of the mRNAs was assessed by electrophoresison 5% polyacrylamide gels containing 7 M urea (30).

To produce capped nv-Rluc RNA, the T7 transcription vector pRL-null (Promega) was linearized with BamHI and then transcribedas described above. The transcripts contain the ORF for Renillaluciferase.

Luciferase expression in infected cells. Capped viral analog RNAs encoding firefly luciferase and nonviral RNAs encoding Renilla luciferase were cotransfected intorotavirus-infected MA104 cells at 1 h p.i. using lipofectAMINE(Life Technologies) (4). At 9 h p.i., the cells were lysedin 1× Passive Lysis Buffer (provided in the Dual Luciferase Kit[Promega]). The levels of firefly and Renilla luciferase activitiesin the lysates were assayed with a Turner TD-20E luminometer (4).

Nuclestide sequence accession numbers. The GenBank accession numbers of the gene 5 cDNAs are AF290881 (30-19), AF290882 (30-1A), AF290883 (4F), and AF290884(5S).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

SA11 variants with novel genotypes. Rotavirus strains SA11-FEM and SA11-4F were serially passaged greater than 20 times at high MOI in MA104 cells. Followingthe emergence of one or more novel dsRNAs in the virus population,the variants 30-1A and 5S were isolated. 30-1A was derived fromSA11-FEM, and its genome lacked a wild-type gene 5 dsRNA but containeda large novel dsRNA migrating between gene 1 and 2 dsRNAs uponPAGE (Fig. 1). In comparison, 5S was derived from SA11-4F andits genome, which also lacked a wild-type gene 5 dsRNA, containeda large, novel dsRNA migrating slightly faster than gene 4 dsRNA.Except for the absence of the wild-type gene 5 dsRNAs and thepresence of the novel dsRNAs, the genome segments of the variants30-1A and 5S comigrated precisely with the genome segments oftheir wild-type counterparts 30-19 and 4F, respectively (Fig.1).

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FIG. 1. Genome segments of wild-type viruses 30-19 and 4F and variants 30-1A and 5S. RNAs were recovered from the viruses by phenol-chloroform extraction and ethanol precipitation, resolved by SDS-PAGE, and detected by staining with ethidium bromide. The arrows denote the positions of aberrant genome segments for 30-1A and 5S.

Duplication of sequences in gene 5 dsRNAs. Reverse transcription-PCR was used to prepare cDNAs of the gene 5 dsRNAs of the variants 30-1A and 5S and the wild-type viruses30-19 and 4F. Nucleotide sequencing of the cDNAs showed that thegene 5 dsRNAs of the wild-type viruses 30-19 and 4F were 1614and 1610 nt in length, respectively, and shared 98 to 99% identitywith the previously reported sequences of the SA11 gene 5 dsRNA(12, 25). The wild-type gene 5 dsRNAs contained single longORFs of 1,488 nt (residues 31 to 1518), 5' UTRs of 30 nt, and3' UTRs of 96 nt for 30-19 and 92 nt for 4F. The protein product,NSP1, encoded by the wild-type gene 5 dsRNAs was predicted tobe of 496 amino acids (aa) (Fig. 2), to have a molecular massof 59 kDa and to share 97 to 98% identity with the NSP1 encodedby other SA11 rotaviruses (12, 25).

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FIG. 2. Alignment of the predicted amino acid sequences of NSP1 encoded by the gene 5 dsRNAs of wild-type viruses 30-19 and 4F and variants 30-1A and 5S. Sequence identity is indicated with dots.

The gene 5 dsRNA of the 30-1A variant was 2,729 nt in length and contained a 1,114-nt duplication of the sequence from residues143 to 1256 of the 30-19 gene 5 dsRNA (Fig. 3). In comparisonto the three other gene 5 dsRNAs containing sequence duplicationswhich have been molecularly described, i.e., brvA (10), brvE(40), and IGV-80-3-re (17) (Fig. 3), the overall length ofthe 30-1A gene 5 dsRNA is the second longest. In the 30-1A gene5 dsRNA, the copies of the duplicated sequences are located atresidues 143 to 1256 and 1258 to 2371 and are separated by a singleT residue (Fig. 4). The origin of the T is not known, but basedon comparison with the sequence of the 30-19 gene 5 dsRNA, theresidue was not specified by the template strand during RNA synthesisand, therefore, was likely generated by an error of the RdRP.The presence of the T at the junction site causes a shift in thereading frame, which results in the addition of five incorrectamino acids to the growing NSP1 polypeptide and in its prematuretermination at nt 1271. The C-truncated NSP1 encoded by 30-1Agene 5 dsRNA is 414 aa in length (Fig. 2), has a molecular massof 49 kDa, and lacks the last 82 aa of wild-type NSP1.

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FIG. 3. Sequence organization of aberrant gene 5 dsRNAs of rotavirus. The lengths of the aberrant gene 5 dsRNAs and their NSP1 products are given, as well as the corresponding values for wild-type gene 5 dsRNAs and their NSP1 products (in parentheses). Regions representing the 5' and 3' UTRs of the wild-type dsRNA are shown with diagonal lines. The sizes and positions of duplicated sequences in the gene 5 dsRNAs of SA11 30-1A, SA11-5S, brvE, brvA, and IGV-80-3-re and deleted sequences in the gene 5 dsRNAs of UK-P9 $Delta$ 5 and A5-16 and the locations of nonsense mutations in the gene 5 dsRNAs of brvA and A5-10 are indicated. The accession numbers for the gene 5 homologs are AF290882 (SA11 30-1A), AF290884 (SA11-5S), Z24735 (brvE, junction sequence only), L12248 (brvA), AF190169 (IGV-80-3-re), Z24736 (UK-P9 $Delta$ 5), D38149 (A5-16), and D38147 (A5-10).

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FIG. 4. Junction of the duplicated sequences in the gene 5 dsRNAs of SA11 30-1A and SA11-5S. The junction of the duplicated sequences includes one (30-1A) or three (5S) nontemplated T residues. Aligned with each junction are the sequences of the wild-type gene 5 dsRNAs of SA11 30-19 or SA11-4F. The alignment indicates the potential sites where the viral RdRP and nascent RNA dissociated from the wild-type RNA template and then, at an upstream site on the same template, reassociated and reinitiated RNA synthesis using the nascent RNA as a primer. The arrowed line illustrates the movement of the RdRP along the wild-type sequence and the synthesis of the nontemplated T residues required to generate the junction sequence during plus-strand synthesis. Repeated sequences near the site where the RdRP is proposed to have dissociated from the wild-type template are overlined. Identity between the 3'-terminal sequence of the nascent transcript and the sequence near where the RdRP reinitiated transcription is also shown.

Sequencing revealed that the gene 5 dsRNA of the variant 5S was 2,162 nt in length and contained a rearrangement resultingfrom a 549-nt duplication of the sequence between residues 917and 1465 of the 4F gene 5 dsRNA (Fig. 3). The two copies of theduplicated sequences are located at residues 917 to 1465 and 1469to 2017 and are separated by a stretch of three Ts (Fig. 4). Aswas the case for the single T detected between the duplicatedsequences of the 30-1A gene 5 dsRNA, the origin of the TTT stretchis not apparent based on the sequence of the 4F gene 5 dsRNA andmay represent the addition of nontemplated residues by the RdRP.The presence of TTT at the junction alters the NSP1 ORF such thatthreonine 479 becomes isoleucine and is followed by a terminationcodon (UAA). As a result, the 5S gene 5 dsRNA encodes a C-truncatedNSP1 of 479 aa (Fig. 2) that has a molecular mass of 57 kDa andlacks the last 18 aa of the wild-typeprotein.

Lack of expression of full-length NSP1 by the 30-1A and 5S variants. To verify that the gene 5 dsRNAs of the 30-1A and 5S variants lacked the ability to encode wild-type NSP1, MA104 cells weremock infected or infected with the variants or their wild-typecounterparts and then maintained in the presence of ³⁵S-labeled amino acids. After harvesting, the cytosol and cytoskeletonfractions of the cells were recovered. The radiolabeled proteinsin the fractions were resolved by SDS-PAGE and detected by autoradiography.As shown in Fig. 5A (cytosol), a radiolabeled protein with thesame molecular mass as NSP1 (59 kDa) was present in cells infectedwith wild-type viruses 30-19 and 4F but was absent in cells thatwere mock infected or infected with 30-1A or 5S. The locationsof the C-truncated NSP1 proteins of 30-1A and 5S on the gel werepredicted based on their expected molecular masses and the presenceof novel proteins in the cytoskeleton fractions of 30-1A- and5S-infected cells that were absent in the cytoskeletal fractionsof mock-infected and 30-19- and 4F-infected cells (Fig. 5). Themock-infected and infected cells were also examined for the presenceof NSP1 by Western blot assay using a monospecific polyclonalantiserum made against a peptide representing the C-terminal 19aa of SA11 NSP1 (Fig. 5B). The analysis confirmed that full-lengthNSP1 was produced in cells infected with the wild-type viruses30-19 and 4F but was not produced in mock-infected cells or cellsinfected with the 30-1A or 5S variant. The lack of availabilityof other antisera to SA11 NSP1 prevented us from using Westernblot analysis to confirm the expression of truncated NSP1 in 30-1A-and 5S-infected cells.

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FIG. 5. Expression of truncated NSP1 in cells infected with the variants 30-1A and 5S and wild-type viruses 30-19 and 4F. Mock- or virus-infected MA104 cells which had been maintained in medium containing ³⁵S-labeled amino acids were lysed at 8 h p.i. with Triton X-100, and the cytosol and cytoskeleton fractions of the cell lysates were recovered. (A) ³⁵S-labeled proteins in the fractions were resolved by SDS-PAGE and detected by autoradiography. The suspected positions of wild-type (30-19 and 4F) and C-truncated (30-1A and 5S) NSP1 are indicated with dots. (B) The cytosol fractions described in panel A were resolved by SDS-PAGE, and the proteins were blotted onto nitrocellulose. The blot was probed with antiserum raised against a peptide corresponding to the last 19 aa of SA11 NSP1. Molecular masses were determined by coelectrophoresis of prestained protein markers.

Small-plaque phenotype of the NSP1-defective variants. Propagation of the wild-type virus 30-19 and its variant 30-1A showed that each grew to a titer of ~1 × 10⁷ in MA104 cells. Likewise, the wild-type virus 4F and its variant5S grew equally well in MA104 cells but they each reached a finaltiter that was at least 10-fold greater than that of 30-19 and30-1A (data not shown). The basis for the difference between thetiters of the 30-19 and 30-1A pair and the 4F and 5S pair is notknown. However, the fact that each of the wild-type viruses andits variant counterpart grew to the same titer indicated thatthe inability to encode full-length NSP1 did not affect virusyield.

In contrast, the diameters of the plaques produced by the 30-1A and 5S variants were approximately one-half of those of theplaques produced by the corresponding wild-type viruses (Table1). Except for P9 $Delta$ 5, whose plaque phenotype has not been reported(38), a decrease in plaque size has also been observed for allvariants that encode defective NSP1. This is the case regardlessof whether the gene 5 dsRNA encoding the defective protein containsa sequence duplication (30-1A, 5S, brvA, and brvE [40]), a sequencedeletion (A5-16 [(38)]), or a nonsense mutation within the NSP1ORF (A5-10 [38]) (Fig. 3). Thus, although NSP1-defective rotavirusescan grow to the same final titer as rotaviruses producing wild-typeNSP1, the inability to produce wild-type NSP1 apparently confersa relatively small-plaque phenotype on the virus. The small-plaquephenotype cannot be correlated with the size of the gene 5 dsRNA.Notably, the plaque size of the IGV-80-3-re variant, which containsa 1.2-kb duplication but encodes full-length NSP1 (17), doesnot differ significantly from IGV isolates containing a wild-typegene 5 dsRNA (K. Kojima, personal communication).

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TABLE 1. Plaque sizes of wild-type SA11 rotavirus and SA11 variants encoding C-truncated NSP1

Absence of the 3' consensus sequence in SA11 gene 5 dsRNAs. While the 3'-terminal sequence of the plus-strand RNAs of nearly all group A rotaviruses is 5'-UGACC-3', sequencing of multiplecDNA clones obtained by rapid amplification of cDNA 5' ends ofthe 3' termini of the gene 5 dsRNAs of the wild-type viruses 30-19and 4F and variants 30-1A and 5S showed that they ended with thesequence 5'-UGAACC-3' (data not shown). Similar analysis of the3' end of gene 5 dsRNA of an SA11-4F isolate obtained from R.F. Ramig (Baylor College of Medicine) showed that it too containedthe nonconsensus sequence UGAACC (data not shown). Given thatMitchell and Both (25) determined that the gene 5 dsRNAs oftheir SA11 isolate ended with this same unusual sequence, we concludethat a feature common to the gene 5 segments of all SA11 strainsof rotavirus is the presence of the atypical 3' -terminal sequenceUGAACC. Sequencing of the gene 5 dsRNAs of the human KU and canineK9 strains have revealed that they too end with the atypical sequenceUGAACC (27). But sequencing of the gene 5 dsRNAs of the bovineA5 (38), RF (34), UK (data not shown), rhesus RRV (date notshown), and avian PO-13 (GenBank accession no. AB009633) strainsof rotavirus has shown that they end with the consensus sequenceUGACC. Thus, the atypical 3' end found for the SA11 gene 5 dsRNAappears to be a feature that is found for the gene 5 dsRNAs ofsome, but not all, strains of rotavirus. While there are manygene 5 sequences in the GenBank database, the 3'-terminal sequencesof most of these were not directly determined. Instead, the reported3'-terminal sequence of the gene 5 RNAs represents the primerthat was used to prepare cDNAs of the gene by reverse trancription-PCR.Therefore, it remains unclear whether the atypical 3' sequenceis a common or a rare feature of rotavirus gene 5dsRNAs.

Atypical 3'-terminal sequence reduces efficiency of gene 5 dsRNA synthesis in vitro. In vitro assays performed with the open-core replication system have shown that the 3' consensus sequence contains a cis-actingsignal that promotes the synthesis of minus-strand RNA (31,42). Site-specific mutagenesis has revealed that modificationsmade to the 3' consensus sequence can reduce the efficiency ofminus-strand synthesis (2). To determine whether the atypical3' end of SA11 gene 5 dsRNA differed from the 3' consensus sequencein the ability to promote minus-strand synthesis, two types ofSA11 gene 5 mRNAs were prepared which were identical in sequenceexcept that one ended with UGAACC and the other ended with UGACC.The two types of mRNAs were separately incubated in the open-coresystem in the presence of [³²P]UTP, and the radiolabeled gene 5 dsRNA products of the assayswere resolved by PAGE and quantified by phosphorimaging. The resultsshowed that the gene 5 mRNA ending with UGAACC was replicatedto approximately one-half of the level of the gene 5 mRNA endingwith the 3' consensus sequence UGACC (Fig. 6). This same differencewas observed regardless of the amount of gene 5 template RNA oropen cores added to the reaction mixtures. Thus, based on thisassay, the presence of GAACC at the end of the gene 5 mRNAs ofSA11 rotavirus significantly reduces the efficiency by which theviral RdRP can replicate the RNA. However, the fact that the atypicalsequence is present in the genome of a nondefective rotaviruswhich can grow to high titer in cell culture indicates that thechange in replication efficiency does not have a marked impacton the ability of the virus to propagate.

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FIG. 6. Effect of the UGACC $right-arrow$ UGAACC mutation on the efficiency of minus-strand synthesis. SA11 gene 5 mRNAs were prepared that ended with the 3' consensus sequence UGACC (GACC) or the atypical sequence UGAACC (GAACC) and used as templates for the synthesis of minus-strand RNA in the open-core replication system. Reaction mixtures contained various amounts of template RNA (A) or open cores (B) and included [³²P]UTP to radiolabel RNA products. ³²P-labeled dsRNA products were detected by SDS-PAGE and autoradiography, and the relative levels of dsRNA products were quantified with a PhosphorImager. The percent GAACC/GACC was calculated by dividing the amount of dsRNA product made in reactions containing template RNA ending with UGAACC by the amount of that ending with UGACC and multiplying the result by 100.

NSP3 recognizes the atypical 3'-terminal sequence. In addition to containing a cis-acting signal that promotes minus-strand synthesis, the 3' consensus sequence also containsan element that enhances translation of rotavirus mRNAs (4).In particular, the last 4 nt of the consensus sequence, GACC,constitute a translation enhancer that is specifically recognizedby NSP3, a nonstructural protein that upregulates gene expressionby promoting circularization of viral mRNAs (34, 35). Thefact that MA104 cells infected with the SA11 wild-type viruses30-19 and 4F produced NSP1 (Fig. 5) demonstrates that viral mRNAswhich lack the precise NSP3 recognition element can be translated.To determine whether NSP3 was able to recognize the atypical 3'end of the SA11 gene 5 mRNA (UGAACC), rNSP3 containing an N-terminalHis tag was expressed in bacteria and purified to homogeneitywith a Ni affinity column (Fig. 7). The rNSP3 was then incubatedwith the ³²P-labeled RNA probe v40-GACC, v40 $Delta$ 3'-11, or v40-GAACC, and themixtures were analyzed for the formation of rNSP3-probe complexesby gel mobility shift assay. The 3' end of the v40-GACC probecorresponds to the last 40 nt of the SA11 gene 8 mRNA and endswith the 3' consensus sequence UGACC. The v40 $Delta$ 3'-11 probe is thesame, except that it lacks the last 11 nt of the v40-GACC probe.Instead of ending with UGACC, the v40-GAACC probe ends with UGAACC.The gel mobility shift analysis showed that rNSP3 formed a complexwith v40-GACC but not with v40 $Delta$ 3'-11 (Fig. 8A). This is consistentwith earlier studies showing that the recognition element forNSP3 is located at the 3' end of viral mRNAs (35). The analysisalso showed that rNSP3 bound not only to v40-GACC but to v40-GAACCas well (Fig. 8B). However, quantitation of the results revealedthat the level of NSP3-probe complexes formed with v40-GAACC wasapproximately one-third of that formed with v40-GACC (data notshown). These data suggest that while the 3' GAACC sequence ofSA11 gene 5 mRNAs does not contain the precise recognition elementfor NSP3, the protein retains the ability to bind specificallyto the 3' end of the mRNA but with decreased affinity.

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FIG. 7. Isolation of His-tagged rNSP3 expressed in bacteria. Protein markers (lane 1) and His-tagged rNSP3, purified with a Ni-nitrilotriacetic acid agarose column (lane 2), were resolved by SDS-PAGE and detected by staining with Coomassie blue R-250.

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FIG. 8. Impact of the UGACC $right-arrow$ UGAACC mutation on the RNA-binding activity of NSP3. Complexes formed by incubating purified rNSP3 with the ³²P-labeled RNA probes v40-GACC and v40 $Delta$ 3'-11 (A) or v40-GACC and v40-GAACC (B) were resolved by electrophoresis on a nondenaturing 6% polyacrylamide gel and detected by autoradiography. The intensity of bands representing rNSP3-probe complexes and free probe were quantified with a PhosphorImager. The values were used to calculate the percentage of probe binding to rNSP3.

Atypical 3'-terminal sequence reduces efficiency of gene expression. Chimeric RNAs, which contained the ORF for firefly luciferase and the UTRs either of SA11 gene 6 mRNA or of nonviral mRNAswere used previously to identify and characterize the rotavirus3' translation enhancer (4). We employed this same system toaddress the question of whether the translational efficiency ofthe SA11 gene 5 mRNAs was reduced because they ended with GAACCinstead of the 3' translation enhancer GACC. To perform this analysis,5'-capped chimeric reporter RNAs were made that contained theORF for firefly luciferase and either the 5' and 3' UTRs of SA11gene 6 mRNA (g6-Fluc-UGACC) or the 5' UTR of $beta$ -globin mRNA andthe 3' UTR of SA11 gene 6 mRNA (glo/g6-Fluc-UGACC). Two derivativesof these chimeric RNAs were also prepared in which the 3'-terminalUGACC sequences were replaced with UGAACC (g6-Fluc-UGAACC andglo/g6-Fluc-UGAACC). Finally, a capped but nonpolyadenylated reporterRNA (nv-Rluc) was prepared that encodes Renilla luciferase andcontains UTRs of nonviral origin. Each of the g6-Fluc and glo/g6-FlucRNAs was then individually cotransfected with nv-Rluc RNA intoSA11 rotavirus-infected MA104 cell at 1 h p.i. At 9 h posttransfection,the levels of firefly and Renilla luciferases expressed in thecells were determined with a luminometer. To compensate againstpossible variations in transfection efficiency, the values obtainedfor the expression of firefly luciferase were then normalizedagainst the values obtained for the expression of Renilla luciferase.The results showed that cells transfected with g6-Fluc-GACC andglo/g6-Fluc-GACC produced approximately four times as much fireflyluciferase as cells transfected with g6-Fluc-GAACC and glo/g6-Fluc-GAACC,respectively (Fig. 9). Thus, mutation of the terminal sequencefrom GACC to GAACC caused a significant decrease in the expressionof the ORF of the chimeric RNAs, suggesting that the mutationpartially inactivated the 3'-terminal enhancer. Consistent withan earlier report (4), the results also showed that the effectof the 3'-terminal sequences of the chimeric RNAs on gene expressionwas not influenced by the 5' UTR. In summary, these data provideindirect evidence that the atypical 3'-terminal sequence on themRNAs of SA11 gene 5 dsRNA probably has a negative effect on theexpression of NSP1 from these mRNAs.

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FIG. 9. Effect of the UGACC $right-arrow$ UGAACC mutation on protein expression in infected cells. The chimeric reporter RNAs g6-Fluc-UGACC and -UGAACC and glo/g6-Fluc-UGACC and -UGAACC were separately cotransfected with nv-Rluc into SA11-infected MA104 cells at 1 h p.i. At 9 h p.i., the levels of firefly and Renilla luciferases per milligram of cell lysate were determined and the expression of firefly luciferase was normalized to the expression of Renilla luciferase. To ease the comparison of values, the expression of firefly luciferase for the g6-Fluc-UGACC and glo/g6-Fluc-UGACC RNAs was set to 100%.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Role of NSP1 in the viral life cycle. With the completion of this study, a total of eight aberrant gene 5 dsRNAs of rotavirus have been molecularly described. Ofthese, five contain sequence duplications (SA11 30-1A, SA11-5S,brvA, brvE, and IGV-80-3-re), two contain sequence deletions (UK-P9 $Delta$ 5and A5-16), and two contain nonsense mutations (brvA and A5-10).Of the eight aberrant gene 5 dsRNAs, only that of the variantIGV-80-3-re encodes full-length NSP1. In contrast, analysis ofthe plaques produced by the variants encoding defective NSP1 hasso far revealed that they are significantly smaller than thoseproduced by the corresponding wild-type viruses, regardless ofwhether the variant contained a large (e.g., SA11 30-1A) or asmall (e.g., A5-16) gene 5 dsRNA. These results indicate thatalthough NSP1 is nonessential, the protein does affect the plaquephenotype of the virus and therefore does have a role in the biologyof the virus when it is propagated in cell culture. Notably, thevariant SA11-5S produced a C-truncated NSP1 that was missing onlythe last 17 aa of the full-length protein. The fact that the plaquesize of this variant was one-half of that of its wild-type counterpartsuggests that even deletion of a relatively few amino acids fromthe C terminus of NSP1 alters the protein's function and resultsin a change in the plaque phenotype of the virus. Thus, the completeNSP1 protein, or nearly all of it, is apparently required to conferthe normal plaque phenotype on the virus. It was also observedthat although SA11 30-1A and SA11-5S produced smaller plaquesthan their wild-type counterparts, MA104 cells infected with thesevariants grew to the same final titer as cells infected with thewild-type viruses. Given the growth and plaque characteristicsof the variants, it may be proposed that defects in NSP1 increasethe length of the viral life cycle (and thereby produce slower-growingplaques) but do not affect the number of progeny virions generatedin the infectedcell.

Mechanism of sequence rearrangement. Previous analysis of a rotavirus variant containing a sequence duplication in the gene 11 dsRNA has provided evidence thatintragenic rearrangements can occur during viral transcription(16). The molecular events leading to rearrangements are notknown. However, it has been proposed that during plus-strand synthesis,the RdRP and nascent transcript detach from the dsRNA templateand then move together to a distant site on the same templatewhere the RdRP reinitiates plus-strand synthesis using the nascenttranscript as a primer (6, 16).

Inspection of the sequences of the atypical gene 5 dsRNAs suggests that during plus-strand synthesis, the RdRP can disengagefrom all regions of the dsRNA template, including near the 5'end (A5-16), the middle (brvE), and the 3' end (IGV-80-3-re) (Fig.3). The RdRP is able to re-engage and reinitiate RNA synthesisat sites that are upstream (e.g., A5-16) or downstream (e.g.,SA11-5S) of the sites at which the RdRP disengaged, and thereby,the RdRP is able to create deletions or duplications, respectively,within the product RNA. The distances between the sites wherethe polymerase disengages and re-engages the template are quitevariable, ranging from 0.3 kb for UK-P9 $Delta$ 5 to 1.2 kb for IGV-80-3-re.As revealed by the analysis of the site at which the RdRP disengagedfrom the gene 5 dsRNA of 30-19, in generating the rearranged gene5 dsRNA of 30-19 (Fig. 4A), repeated sequences of significantlength need not be present for the polymerase to release fromthe RNA template. Similarly, for the disengaged RdRP to reinitiateRNA synthesis elsewhere on the dsRNA template using the nascentRNA as a primer, the 3' end of the nascent RNA need not have extensivecomplementarity with sequences of the template at or near thesite of reinitiation (Fig. 4A).

During the rearrangement of the gene 5 dsRNAs of the variants 30-1A and 5S, one or three nontemplated T residues, respectively,were introduced at the junction site of the duplicated sequences(Fig. 4). An important but unanswerable question is whether theT residues were added before or after the RdRP disengaged fromthe template. If before, then the presence of the nontemplatedresidues may have destabilized the interaction between the nascentRNA and the RNA template at the transcription fork, causing therelease of the nascent strand and RdRP. However, the fact thatgene 5 rearrangements have been described which lack any notablenontemplated nucleotides at the junction site suggests that otherevents are also involved in causing the RdRP to disengage fromthe RNAtemplate.

Basis for selection of RNAs containing sequence duplications. All of the variants shown in Fig. 3 that contain duplicated gene 5 sequences emerged during passage of wild-type rotavirusesat high MOI. The increasing predominance of the rearranged gene5 dsRNA as the virus lysates were serially passaged indicatesthat there was a selective advantage in their use in the virallife cycle over the wild-type gene 5 dsRNA. Indeed, analysis ofcells coinfected with equal amounts of wild-type virus and variantswith duplicated sequences in gene 5 or 11 has also suggested thatdsRNAs with sequence duplications have a selective advantage overthose that do not (5, 13). Since rotavirus mRNAs are believedto undergo selection (assortment) and packaging into cores priorto replication into dsRNAs, it is reasonable to propose that,in fact, the sequence rearrangement alters the mRNA in a way that,directly or indirectly, increases the frequency by which the mRNAis assorted and/or packaged. The nature of the advantage is unclearbut simply may be related to an increase in the overall size ofthe transcripts made from gene 5 dsRNAs containing sequence duplications.Alternatively, it is possible that the increase in the lengthof the 3' UTR generated by the sequence rearrangement in itselfprovides a selective advantage. The increased size of the transcriptor its 3' UTR may make it more difficult for NSP3 to cause thecircularization of the mRNAs and, thereby, for the mRNAs to berecruited into polysomes. As a consequence, the probability mayincrease that the transcripts interact with those viral RNA-bindingproteins that target their movement to viroplasms and their introductioninto replicationintermediates.

Importance of the 3' consensus sequence for RNA replication and gene expression. It was found that the 3'-terminal sequence of the gene 5 dsRNAs of all isolates of SA11 rotaviruses was UGAACC and not theexpected consensus sequence UGACC. Our analyses indicate thatthe A insertion into the consensus sequence affects the abilityof rotavirus mRNAs to serve as templates for minus-strand synthesis,to be recognized by NSP3, and to be efficiently translated. Basedon assays performed with the open-core replication system, theUGAACC sequence is only 50% as efficient in promoting dsRNA synthesisas the UGACC sequence. However, since SA11 viruses grow to hightiter (>10⁸) and have relatively large-plaque phenotypes, the negative impactthat the atypical 3' end has on the replication of the gene 5mRNA is not necessarily significant to the biology of these viruses.In terms of using the open-core system as a tool for identifyingsequences in viral mRNAs that promote minus-strand synthesis,our results indicate that mutations made in viral mRNAs that reduceminus-strand synthesis in vitro by 50% cannot be interpreted asrepresenting changes that would render a virusnonviable.

Gel shift assays demonstrated that SA11 NSP3 specifically recognizes the atypical 3' sequence UGAACC of SA11 gene 5 dsRNA,although less efficiently than the 3' consensus sequence UGACC.This result is contrary to previous results which indicated thatthe four-base sequence GACC was necessary and sufficient for interactionwith NSP3. In particular, Poncet et al. (35) reported that NSP3was not able to form complexes with UAACC but was able to formcomplexes with GGACC, suggesting that in their studies the G residueat $-$ 4 was critical for recognition by NSP3. In their studies,the probe UGAACC was not tested. The difference between our resultsand those of Poncet et al. (35) may stem from minor differencesin specificity between SA11 NSP3 and bovine NSP3. Even thoughthe gene 5 dsRNA of SA11 lacked the 3' consensus sequence, cellsinfected with the virus expressed NSP1. Thus, despite the proposedimportance of the 3' consensus sequence in viral mRNA circularizationand gene expression, the sequence, in fact, is not required fortranslation of viralmRNAs.

If the 3' sequence UGAACC functions suboptimally in promoting dsRNA synthesis and gene expression, then why does it existin SA11 gene 5 dsRNAs? The simplest answer is that it leads tolower expression of NSP1 in infected cells. The frequency at whichgene 5 rearrangements occur and then dominate over wild-type gene5 RNAs during serial passage of the rotaviruses in cell cultureindicates that viruses which no longer encode wild-type NSP1 mayhave a selective advantage over those that do. If this is true,then it is reasonable to presume that an A insertion into thegene 5 3' consensus sequence may confer an advantage on the SA11virus because it partially inactivates the 3' translation enhancerand, as a result, decreases the expression of wild-type NSP1.In this scenario, the selective advantage in favor of inactivatingthe 3' translation enhancer would be dominant over any deleteriouseffect that the A insertion would have on the ability of the 3'sequence to promote minus-strandsynthesis.

	ACKNOWLEDGMENTS

V.G. was supported in part by a fellowship from CNPq, Brasilia, Brazil, and by a grant from FAPERJ, Rio de Janeiro,Brazil.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases,National Institutes of Health, 7 Center Dr., MSC 0720, Room 117,Bethesda, MD 20892. Phone: (301) 496-3372. Fax: (301) 496-8312.E-mail: jpatton{at}atlas.niaid.nih.gov.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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21. Malherbe, H. H., and M. Strickland-Cholmley. 1967. Simian virus SA11 and the related O agent. Arch. Gesamte Virusforsch. 22:235-245[CrossRef][Medline].

22. Mattion, N. M., and M. K. Estes. 1991. Sequence of a rotavirus gene 4 associated with unique biologic properties. Arch. Virol. 120:109-113[CrossRef][Medline].

23. McCrae, M. A., and J. G. McCorquodale. 1983. Molecular biology of rotaviruses. V. Terminal structure of viral RNA species. Virology 126:204-212[CrossRef][Medline].

24. Mendez, E., C. F. Arias, and S. Lopez. 1992. Genomic rearrangements in human rotavirus strain WA: analysis of rearranged RNA segment 7. Arch. Virol. 125:331-338[CrossRef][Medline].

25. Mitchell, D. B., and G. W. Both. 1990. Conservation of a potential metal binding motif despite extensive sequence diversity in the rotavirus nonstructural protein NS53. Virology 174:618-621[CrossRef][Medline].

26. Nishikawa, K., K. Taniguchi, A. Torres, Y. Hoshino, K. Green, A. Z. Kapikian, R. M. Chanock, and M. Gorziglia. 1988. Comparative analysis of the VP3 gene of divergent strains of the rotaviruses simian SA11 and bovine Nebraska calf diarrhea virus. J. Virol. 62:4022-4026[Abstract/Free Full Text].

27. Okada, J., N. Kobayashi, K. Taniguchi, and H. Shiomi. 1999. Functional analysis of the heterologous NSP1 genes in the genetic background of simian rotavirus SA11. Arch. Virol. 144:1439-1449[CrossRef][Medline].

28. Patton, J. T. 1996. Rotavirus VP1 alone specifically binds to the 3' end of viral mRNA, but the interaction is not sufficient to initiate minus-strand synthesis. J. Virol. 70:7940-7947[Abstract].

29. Patton, J. T., and E. Spencer. 2000. Differences and similarities in RNA replication of viruses with segmented double-stranded RNA genomes. Virology 277:217-225[CrossRef][Medline].

30. Patton, J. T., Z. Taraporewala, V. Chizhikov, and D. Chen. 1999. Virus replication. Methods Mol. Med. 34:33-66.

31. Patton, J. T., M. Wentz, J. Xiaobo, and R. F. Ramig. 1996. cis-acting signals that promote genome replication in rotavirus mRNA. J. Virol. 70:3961-3971[Abstract].

32. Pedley, S., F. Hundley, I. Chrystie, M. A. McCrae, and U. Desselberger. 1984. The genomes of rotaviruses isolated from chronically infected immunodeficient children. J. Gen. Virol. 65:1141-1150[Abstract/Free Full Text].

33. Pereira, H. G., R. S. Azeredo, A. M. Fialho, and M. N. P. Vidal. 1984. Genomic heterogeneity of simian rotavirus SA11. J. Gen. Virol. 65:815-818[Abstract/Free Full Text].

34. Piron, M., P. Vende, J. Cohen, and D. Poncet. 1998. Rotavirus RNA-binding protein NSP3 interacts with eIF4GI and evicts the poly(A) binding protein from eIF4F. EMBO J. 17:5811-5821[CrossRef][Medline].

35. Poncet, D., S. Laurent, and J. Cohen. 1994. Four nucleotides are the minimal requirement for RNA recognition by rotavirus non-structural protein NSP3. EMBO J. 13:4165-4173[Medline].

36. Shen, S., B. Burke, and U. Desselberger. 1994. Rearrangement of the VP6 gene of a group A rotavirus in combination with a point mutation affecting trimer stability. J. Virol. 68:1682-1688[Abstract/Free Full Text].

37. Spencer, E., and M. L. Arias. 1981. In vitro transcription catalyzed by heat-treated human rotavirus. J. Virol. 40:1-10[Abstract/Free Full Text].

38. Taniguchi, K., K. Kojima, and S. Urasawa. 1996. Nondefective rotavirus mutants with an NSP1 gene which has a deletion of 500 nucleotides, including a cysteine-rich zinc finger motif-encoding region (nucleotides 156 to 248), or which has a nonsense codon at nucleotides 153 to 155. J. Virol. 70:4125-4130[Abstract].

39. Taraporewala, Z., D. Chen, and J. T. Patton. 1999. Multimers formed by the rotavirus nonstructural protein NSP2 bind to RNA and have nucleoside triphosphatase activity. J. Virol. 73:9934-9943[Abstract/Free Full Text].

40. Tian, Y., O. Tarlow, A. Ballard, U. Desselberger, and M. A. McCrae. 1993. Genomic concatemerization/deletion in rotaviruses: a new mechanism for generating rapid genetic change of potential epidemiological importance. J. Virol. 67:6625-6632[Abstract/Free Full Text].

41. Vende, P., M. Piron, N. Castagne, and D. Poncet. 2000. Efficient translation of rotavirus mRNA requires simultaneous interaction of NSP3 with the eukaryotic translation initiation factor eIF4G and the mRNA 3' end. J. Virol. 74:7064-7071[Abstract/Free Full Text].

42. Wentz, M. J., J. T. Patton, and R. F. Ramig. 1996. The 3'-terminal consensus sequence of rotavirus mRNA is the minimal promoter of negative-strand RNA synthesis. J. Virol. 70:7833-7841[Abstract].

Journal of Virology, March 2001, p. 2076-2086, Vol. 75, No. 5
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.5.2076-2086.2001

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3.	Chen, D., C. Q.-Y. Zeng, M. J. Wentz, M. Gorziglia, M. K. Estes, and R. F. Ramig. 1994. Template-dependent, in vitro replication of rotavirus RNA. J. Virol. 68:7030-7039[Abstract/Free Full Text].
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19.	Lawton, J. A., C. Q.-Y. Zeng, S. K. Mukherjee, J. Cohen, M. K. Estes, and B. V. V. Prasad. 1997. Three dimensional analysis of recombinant rotavirus-like particles with intact and amino-terminal-deleted VP2: implications for the architecture of the VP2 capsid layer. J. Virol. 71:7353-7360[Abstract].
20.	Liu, M., P. A. Offit, and M. K. Estes. 1988. Identification of the siman rotavirus SA11 genome segment 3 product. Virology 162:26-32.
21.	Malherbe, H. H., and M. Strickland-Cholmley. 1967. Simian virus SA11 and the related O agent. Arch. Gesamte Virusforsch. 22:235-245[CrossRef][Medline].
22.	Mattion, N. M., and M. K. Estes. 1991. Sequence of a rotavirus gene 4 associated with unique biologic properties. Arch. Virol. 120:109-113[CrossRef][Medline].
23.	McCrae, M. A., and J. G. McCorquodale. 1983. Molecular biology of rotaviruses. V. Terminal structure of viral RNA species. Virology 126:204-212[CrossRef][Medline].
24.	Mendez, E., C. F. Arias, and S. Lopez. 1992. Genomic rearrangements in human rotavirus strain WA: analysis of rearranged RNA segment 7. Arch. Virol. 125:331-338[CrossRef][Medline].
25.	Mitchell, D. B., and G. W. Both. 1990. Conservation of a potential metal binding motif despite extensive sequence diversity in the rotavirus nonstructural protein NS53. Virology 174:618-621[CrossRef][Medline].
26.	Nishikawa, K., K. Taniguchi, A. Torres, Y. Hoshino, K. Green, A. Z. Kapikian, R. M. Chanock, and M. Gorziglia. 1988. Comparative analysis of the VP3 gene of divergent strains of the rotaviruses simian SA11 and bovine Nebraska calf diarrhea virus. J. Virol. 62:4022-4026[Abstract/Free Full Text].
27.	Okada, J., N. Kobayashi, K. Taniguchi, and H. Shiomi. 1999. Functional analysis of the heterologous NSP1 genes in the genetic background of simian rotavirus SA11. Arch. Virol. 144:1439-1449[CrossRef][Medline].
28.	Patton, J. T. 1996. Rotavirus VP1 alone specifically binds to the 3' end of viral mRNA, but the interaction is not sufficient to initiate minus-strand synthesis. J. Virol. 70:7940-7947[Abstract].
29.	Patton, J. T., and E. Spencer. 2000. Differences and similarities in RNA replication of viruses with segmented double-stranded RNA genomes. Virology 277:217-225[CrossRef][Medline].
30.	Patton, J. T., Z. Taraporewala, V. Chizhikov, and D. Chen. 1999. Virus replication. Methods Mol. Med. 34:33-66.
31.	Patton, J. T., M. Wentz, J. Xiaobo, and R. F. Ramig. 1996. cis-acting signals that promote genome replication in rotavirus mRNA. J. Virol. 70:3961-3971[Abstract].
32.	Pedley, S., F. Hundley, I. Chrystie, M. A. McCrae, and U. Desselberger. 1984. The genomes of rotaviruses isolated from chronically infected immunodeficient children. J. Gen. Virol. 65:1141-1150[Abstract/Free Full Text].
33.	Pereira, H. G., R. S. Azeredo, A. M. Fialho, and M. N. P. Vidal. 1984. Genomic heterogeneity of simian rotavirus SA11. J. Gen. Virol. 65:815-818[Abstract/Free Full Text].
34.	Piron, M., P. Vende, J. Cohen, and D. Poncet. 1998. Rotavirus RNA-binding protein NSP3 interacts with eIF4GI and evicts the poly(A) binding protein from eIF4F. EMBO J. 17:5811-5821[CrossRef][Medline].
35.	Poncet, D., S. Laurent, and J. Cohen. 1994. Four nucleotides are the minimal requirement for RNA recognition by rotavirus non-structural protein NSP3. EMBO J. 13:4165-4173[Medline].
36.	Shen, S., B. Burke, and U. Desselberger. 1994. Rearrangement of the VP6 gene of a group A rotavirus in combination with a point mutation affecting trimer stability. J. Virol. 68:1682-1688[Abstract/Free Full Text].
37.	Spencer, E., and M. L. Arias. 1981. In vitro transcription catalyzed by heat-treated human rotavirus. J. Virol. 40:1-10[Abstract/Free Full Text].
38.	Taniguchi, K., K. Kojima, and S. Urasawa. 1996. Nondefective rotavirus mutants with an NSP1 gene which has a deletion of 500 nucleotides, including a cysteine-rich zinc finger motif-encoding region (nucleotides 156 to 248), or which has a nonsense codon at nucleotides 153 to 155. J. Virol. 70:4125-4130[Abstract].
39.	Taraporewala, Z., D. Chen, and J. T. Patton. 1999. Multimers formed by the rotavirus nonstructural protein NSP2 bind to RNA and have nucleoside triphosphatase activity. J. Virol. 73:9934-9943[Abstract/Free Full Text].
40.	Tian, Y., O. Tarlow, A. Ballard, U. Desselberger, and M. A. McCrae. 1993. Genomic concatemerization/deletion in rotaviruses: a new mechanism for generating rapid genetic change of potential epidemiological importance. J. Virol. 67:6625-6632[Abstract/Free Full Text].
41.	Vende, P., M. Piron, N. Castagne, and D. Poncet. 2000. Efficient translation of rotavirus mRNA requires simultaneous interaction of NSP3 with the eukaryotic translation initiation factor eIF4G and the mRNA 3' end. J. Virol. 74:7064-7071[Abstract/Free Full Text].
42.	Wentz, M. J., J. T. Patton, and R. F. Ramig. 1996. The 3'-terminal consensus sequence of rotavirus mRNA is the minimal promoter of negative-strand RNA synthesis. J. Virol. 70:7833-7841[Abstract].