Genes Required for Replication of the 15.5-Kilobase RNA Genome of a Plant Closterovirus

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J Virol, July 1998, p. 5870-5876, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Genes Required for Replication of the 15.5-Kilobase RNA Genome of a Plant Closterovirus

Valery V. Peremyslov,¹ Yuka Hagiwara,¹ and Valerian V. Dolja¹^,²^,^*

Department of Botany and Plant Pathology¹ and Center for Gene Research and Biotechnology,² Oregon State University, Corvallis, Oregon 97331

Received 29 December 1997/Accepted 14 April 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

A full-length cDNA clone of beet yellows closterovirus (BYV) was engineered and used to map functions involved in the replicationof the viral RNA genome and subgenomic RNA formation. Among 10open reading frames (ORFs) present in BYV, ORFs 1a and 1b sufficefor RNA replication and transcription. The proteins encoded inthese ORFs harbor putative methyltransferase, RNA helicase, andRNA polymerase domains common to Sindbis virus-like viruses anda large interdomain region that is unique to closteroviruses.The papain-like leader proteinase (L-Pro) encoded in the 5'-proximalregion of ORF 1a was found to have a dual function in genome amplification.First, the autocatalytic cleavage between L-Pro and the remainderof the ORF 1a product was essential for replication of RNA. Second,an additional L-Pro function that was separable from proteolyticactivity was required for efficient RNA accumulation. The deletionof a large, ~5.6-kb, 3'-terminal region coding for a 6-kDa hydrophobicprotein, an HSP70 homolog, a 64-kDa protein, minor and major capsidproteins, a 20-kDa protein, and a 21-kDa protein (p21) resultedin replication-competent RNA. However, examination of mutantswith replacements of start codons in each of these seven 3'-terminalORFs revealed that p21 functions as an enhancer of genome amplification.The intriguing analogies between the genome organization and replicationalrequirements of plant closteroviruses and animal coronavirus-likeviruses are discussed.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The closterovirus family belongs to the Sindbis virus-like supergroup of positive-strand RNA viruses (35), representingfilamentous plant viruses that possess the largest genomes ofthis supergroup (from ~15 to 20 kb). In addition, closterovirusesexhibit striking similarities in genome organization to the phylogeneticallyremote animal coronavirus-like viruses. It was suggested thatthese similarities reflect parallel evolution toward large RNAgenomes (17).

The available information concerning the functions of closterovirus proteins was inferred mainly from computer-assisted analysis.Nine open reading frames (ORFs) were found in the ~15.5-kb genomeof beet yellows virus (BYV), a prototype closterovirus (2-4).The 5'-terminal part of the BYV RNA harbors ORFs 1a and 1b, encodingpapain-like leader proteinase (L-Pro), putative methyltransferase,RNA helicase, and RNA polymerase domains (Fig. 1A). Among theSindbis virus-like viruses, closteroviruses are distinguishedby a large interdomain region present in ORF 1a and by the apparentinvolvement of a +1 translational frameshift for expression ofthe ORF 1b product (4).

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FIG. 1. (A) Gene organization of BYV and summary of the introduced mutations. L-Pro, papain-like leader proteinase (the arrow shows the site of L-Pro-mediated cleavage); MET and HEL, putative methyltransferase and RNA helicase domains in the ORF 1a product; POL, putative RNA polymerase; HSP70h, an HSP70 homolog; CPm and CP, the minor and major capsid proteins, respectively; p6, p64, p20, and p21, the 6-, 64-, 20-, and 21-kDa products of ORFs 2, 4, 7, and 8, respectively. Asterisks denote replacement of the start codons in each of ORFs 2 to 8; fs, frameshift mutation. AN, SB, and SS, expanded deletions in the 3'-terminal part of the BYV genome. (B) Diagrammatic representation of the full-length BYV-Cal cDNA flanked by the SP6 RNA polymerase promoter in pBYV-NA. The most 5'-terminal and 3'-terminal trinucleotides in the BYV cDNA are shown. The SmaI restriction endonuclease site engineered downstream from the BYV cDNA (boldface) and selected sites used for cloning and mutagenesis are indicated above the diagram, together with their positions in the genome (kilobases). Four BYV cDNA fragments used to generate pBYV-NA are shown as double lines above the diagram. The boundaries of the five cDNA subclones engineered for site-directed mutagenesis are marked below the diagram.

The 3'-terminal part of the BYV genome encompasses ORFs 2 through 8, coding for a 6-kDa hydrophobic protein (p6), a homologof cellular molecular chaperones from the HSP70 family (HSP70h),a 64-kDa protein (p64), two capsid proteins, a 20-kDa protein(p20), and a 21-kDa protein (p21; Fig. 1A) (2, 3, 7).Unlike all of the other elongated plant viruses assembled froma single type of capsid protein, closterovirus particles possessmajor and minor capsid proteins that form a long "body" and ashort "tail" (CP and CPm, respectively; reference 5).

All ORFs located in the 3'-terminal parts of the related genomes of BYV and citrus tristeza closterovirus (CTV) are expressedvia formation of a nested set of subgenomic RNAs (sgRNAs) (14,22, 24). The levels and time courses of accumulation of differentsgRNAs are controlled at the transcriptional level (41). Themechanism of closterovirus transcription appears to be similarto that of other Sindbis virus-like viruses (1, 20, 23,29, 39, 40) and does not involve the leader priming thatwas found in coronavirus-like viruses (25, 37, 38, 50,51).

In this study, we engineered a full-length 15.5-kb cDNA clone of BYV and demonstrated that the corresponding RNA transcriptswere infectious after transfection into plant protoplasts. Site-directedmutagenesis was employed to reveal that the products of BYV ORFs1a and 1b are involved in RNA replication. Among these products,L-Pro, encoded in the 5'-proximal region of ORF 1a, was requiredfor efficient genome amplification, whereas products encoded bythe rest of ORF 1a and by ORF 1b were essential for a basal levelof RNA replication. In addition, p21, a product of the 3'-mostBYV ORF, was identified as an enhancer of RNA accumulation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Nucleotide sequencing of the Californian isolate of BYV. The Californian isolate of BYV (BYV-Cal) was obtained from Bryce W. Falk (University of California at Davis) and propagatedon Tetragonia expansa plants. The virions and RNA were isolatedas previously described (26). The double-stranded RNA (dsRNA)was purified by using CF11 cellulose (48). To determine thenucleotide sequences of the 3' extremities of the minus and plusstrands of BYV-Cal RNA, the virion RNA and BYV-specific dsRNAwere polyadenylated in vitro by using yeast poly(A) polymerasein accordance with the manufacturer's (U.S. Biochemical Corp.)protocol. The 911-nucleotide-long 5'-terminal region of the polyadenylatedminus strand of the dsRNA was amplified via reverse transcription(RT)-PCR after denaturation by 20 mM methylmercuric hydroxide(Serva; reference 47). The RT and PCR were carried out by usingSuperScript II reverse transcriptase (Gibco-BRL), Taq DNA polymerase,and Taq Extender (Stratagene) in accordance with the manufacturers'protocols. The primers used for RT-PCR, dTSac (5'-GGTGAGCTC[T]₁₈)and 900Sph (5'-GTTGCATGCTTTATTTATCTTCCG), contained SacI and SphIsites for subsequent cloning of the amplified products into vectorplasmid pGEM-4 (Promega). A similar protocol was used to clonethe 440-nucleotide-long 3'-terminal fragment of polyadenylatedvirion RNA. The primers used were 500Sph (5'-GTGCATGCGTGGTAACTCCTAT)and dTSac. The cloned inserts were sequenced by the dye terminationmethod using SP6 and T7 primers and an ABI Prism model 377 automatedsequencer. The nucleotide sequence of the remaining part of theBYV-Cal genome was determined in a stepwise manner by using afull-length cDNA clone (see below) and sets of plus- and minus-strandoligonucleotide primers designed on the basis of previously determinedfragments of the BYV-Cal nucleotide sequence.

Generation of a BYV genomic cDNA clone. The first variant of the full-length BYV cDNA clone was assembled from three fragments that were amplified by RT-PCR withvirion RNA of BYV-Cal as the template. These three fragments weredelimited by the 5' end, restriction endonuclease SacI and BamHIsites, and the 3' end as shown in Fig. 1B. The 5'-terminal and3'-terminal PCR products were inserted into pGEM-4-based plasmidpTL7SN (42) as EcoRI-SacI and BamHI-SmaI fragments, respectively.The EcoRI and SmaI sites were added to amplification productsby inclusion into PCR primers, whereas the SacI and BamHI siteswere naturally present in BYV-Cal cDNA. The unique SmaI was introduceddownstream from the 3' end of the viral cDNA to permit linearizationof the plasmid prior to transcription (Fig. 1B). The junctionbetween the SP6 RNA polymerase promoter and the 5' terminus ofthe cDNA was repaired by site-directed mutagenesis (36) to ensurethat the 5' end of the corresponding in vitro transcripts wouldbe identical to that of BYV RNA (Fig. 1B). Finally, the centralpart was inserted between the SacI and BamHI sites to form thefull-length BYV clone. This strategy was similar to that usedsuccessfully to generate a full-length cDNA clone of tobacco etchvirus (15).

The RNA transcripts derived from several tested RT-PCR full-length clones produced no infectivity in protoplast transfectionexperiments (data not shown), possibly due to errors introducedby PCR. Because of that, we subsequently replaced all but the5'-terminal 840 nucleotides (position of the BglII site, Fig.1B) of the original clone with DNA obtained via conventional cDNAcloning (the Gibco-BRL protocol for SuperScript II reverse transcriptasewas used). Four partially overlapping fragments of double-strandedcDNA used for that purpose and delimited by BglII, EagI, SnaBI,NdeI, and SmaI sites are shown in Fig. 1B.

Eight individual full-length BYV cDNA clones of the second generation (with various combinations of cDNA fragments) were testedvia transfection of corresponding RNA transcripts into tobaccoprotoplasts. Two of these transcripts were infectious, exhibitingsimilar levels of RNA accumulation (data not shown). Since theauthentic 5' end of BYV cDNA (5'-GTTT) is suboptimal for SP6 RNApolymerase, it was modified to the more optimal 5'-GAAT sequencein a clone designated pBYV-NA. It was found that the yield ofcorresponding in vitro RNA transcripts was substantially increasedwithout affecting the specific infectivity of the transcripts,which was roughly similar to the infectivity of the virion RNA(data not shown). This apparently high infectivity of transcripts,compared to that of virion RNA, could be due to the relativelylow infectivity of the latter. Even the best preparations of thevirion RNA contain a substantial proportion of degradation productsdue to the fragility of long virions and RNA.

Mutagenesis of the BYV genome. Since site-directed mutagenesis (36) of the ~18.5-kb plasmid harboring ~15.5 kb of the viral cDNA was impractical, fiveplasmids that contained different regions of the BYV genome weregenerated by subcloning of the cDNA fragments into pGEM-4 (Fig.1B). Among those, p5'BYV harbored the genome region between nucleotides1 and 3,472 (position of the SacI site), p65M contained the regionbetween nucleotides 8,472 and 11,694 (delimited by two EcoRI sites),pSB-C was cloned in the opposite orientation and delimited bythe SphI site at position 10,568 and the BamHI site at position13,392, pNB contained the region from the NdeI site at position11,309 to the BamHI site, and p3'-BYV harbored a fragment extendingfrom the BamHI site to the SmaI site (Fig. 1B).

The p5'BYV clone was used to introduce mutations into the L-Pro-encoding region. The mutation designated dcl (for deletionof cleavage site) resulted in in-frame replacement of nucleotides1,848 through 1,875 with the unrelated heptanucleotide GAGATCTharboring a BglII site. The replaced sequence included two glycinecodons that form a scissile bond between L-Pro and the rest ofthe ORF 1a product (4). Four additional L-Pro mutations introducedvia "loop-out" mutagenesis represented in-frame deletions of regionscoding for putative structural elements of L-Pro, predicted byusing the PHD program (EMBL, Heidelberg, Germany). The 1DL deletionremoved BYV nucleotides 270 through 345, specifying a putativeproline-rich, 26-residue-long loop. The 2DL deletion removed BYVnucleotides 493 through 564, corresponding to a 24-residue-longregion containing a short $alpha$ -helix. The 3DL deletion removed BYVnucleotides 937 to 1,007, specifying a putative 24-residue-longregion with high solvent accessibility. The 4DL deletion removedBYV nucleotides 1,207 through 1,301, specifying a 32-residue-longregion harboring a short $alpha$ -helix (see Fig. 3A). In each case,the deleted region was replaced with a hexanucleotide comprisinga BglII site.

Larger in-frame deletions were introduced into the L-Pro coding region by removing DNA fragments between the engineered BglIIsites and a natural BglII site located at nucleotide 841. In the1-B, B-4, and 1-4 mutants, regions located between nucleotides270 and 841, 841 and 1,301, and 270 and 1,301, respectively, weredeleted (see Fig. 3A). The DNA fragments from mutant derivativesof p5'BYV were cloned into the full-length clone by using twounique restriction sites, NheI (located in the vector part ofthe plasmid) and EagI (located at nucleotide 2,152).

The frameshift (fs) mutation upstream of the putative RNA helicase domain encoded by ORF 1a was introduced by filling (47)a unique AvrII restriction site located at nucleotide 6,420 (Fig.1A). One large deletion (SS) in the 3' half of the BYV cDNA wasgenerated by removal of the ~4,300-nucleotide fragment of pBYV-NAlocated between the unique SnaBI and StuI restriction sites. Anotherdeletion (SB) spanned an ~4,750-nucleotide region located betweenthe SphI and BstEII sites (Fig. 1A). To generate a third largedeletion, a unique ApaI site was engineered in p65M downstreamfrom the ORF 2 start codon by site-directed mutagenesis. The mutantfragment was cloned into the full-length clone by using the SnaBIand NdeI sites, and a ~5,600-nucleotide region between the ApaIand NsiI sites was deleted to form the AN mutant (Fig. 1A).

A series of start codon replacement mutants was generated by changing the first ATG codon of each of ORFs 2 through 8 by usingsubclones p65M, pSB-C, pNB, and p3'BYV (Fig. 1B). p65M was utilizedto replace start codons in ORFs 2 and 3 with ATA. The start codonof ORF 4 was replaced with ACG by using pSB-C. Analogous mutationof the ORF 5 start codon was done by using pNB. Finally, startcodons in ORFs 6, 7, and 8 were changed to ATA, GTA, and ACG,respectively, by using p3'BYV. Since ORFs 3 and 4, 4 and 5, 6and 7, and 7 and 8 overlap, the start codon replacements weredesigned so as not to result in any amino acid changes in theproducts encoded in the alternative ORFs. The introduced mutationswere verified by nucleotide sequencing. The sequences of the numerousprimers used for engineering and mutagenesis of the BYV cloneare available upon request.

Analyses of BYV mutants. The genome size RNA transcripts were generated under capping conditions by using SmaI-linearized plasmids and SP6 RNA polymerase(Ambion; 16). These transcripts were transfected via electroporationinto protoplasts obtained from a suspension culture of the Nicotianatabacum cv. Xanthi nc cell line developed by D. Facciotti (Calgene,Inc.) and referred to as the DF line (18). Protoplasts wereharvested at 86 h posttransfection, and the RNA samples were isolatedby using TRIZOL reagent (Gibco-BRL). Northern analysis was conductedby using a Zeta-Probe membrane (Bio-Rad). RNA transfer from a1% agarose gel onto a membrane was in 10× SSC (1× SSC is 0.15M NaCl plus 0.015 M sodium citrate) in accordance with reference6a, whereas prehybridization and hybridization were conductedby using NorthernMax buffer (Ambion) at 50°C. ³²P-labeled positive- or negative-polarity single-stranded RNA probeswere prepared by in vitro transcription using SP6 or T7 RNA polymerase(the T7 promoter is located downstream from inserts in all pGEM-4derivatives) and p3'BYV linearized at the BstEII or BamHI site,respectively. The radiolabeled products were detected and quantifiedby using a PhosphorImager (Molecular Dynamics). At least fourindependent protoplast transfection experiments were conductedfor each mutant; the means and standard deviations were used forcomparative analysis of RNA accumulation.

The capped RNA transcripts of p5'BYV derivatives harboring mutations in the L-Pro coding region were generated in vitro byusing SP6 RNA polymerase and KpnI-linearized plasmid DNA (thesite is located at nucleotide 2,813). In vitro translations wereconducted for 1 h by using wheat germ extracts (Promega). Theproducts were labeled with [³⁵S]methionine (Amersham), separated in sodium dodecyl sulfate-containing12% polyacrylamide gels, and electroblotted onto a PROTRAN nitrocellulosemembrane (Schleicher & Schuell). The radioactivity measured inthe bands corresponding to unprocessed or processed translationproducts by using a PhosphorImager was normalized to the numberof methionine residues present in each product and used for comparativeanalysis of the proteolysis efficiency of mutant L-Pro variants.

Nucleotide sequence accession numbers. The complete nucleotide sequence of the full-length BYV-Cal cDNA from which infectious RNA transcripts can be obtained wasdeposited into the GenBank (accession no. AF056575) database.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Sequence variability in the BYV genome. Due to their critical role in RNA replication, we thoroughly characterized the 5'- and 3'-terminal regions of the BYV-Calgenome. The 3' end of the minus strand of viral dsRNA was polyadenylatedin vitro, amplified by RT-PCR, and cloned; the nucleotide sequencesof six clones were determined. The inferred sequence of the 5'-terminalnoncoding region of the plus strand was identical to that of theUkrainian isolate (4) in five clones. One clone deviated byhaving an A instead of a U as the second nucleotide. In addition,all six clones harbored an extra G at the very 3' end of the minus-strandRNA. The presence of an analogous nontemplate G in genomic minusstrands was previously described for several viruses of plants(9, 12, 13), including CTV (27).

Unexpectedly, high sequence variation was found in the 3'-terminal noncoding regions of the two BYV isolates. In place ofthe very 3'-terminal heptanucleotide GGGGCCC_OH found in UkrainianBYV (3), BYV-Cal harbored hexanucleotide GGGCCG_OH in 10 sequencedcDNA clones. In addition, the sequence 5'-C(A)₆(U)₅C(U)₅AUAUUAAG(A)₄(U)₅-3',present in Ukrainian BYV (nucleotides 15,400 to 15,434), was replacedin BYV-Cal with the sequence (A)₆(U)_5-7(A)_7-14 (U)₅,starting at nucleotide 15,401. Among 10 sequenced independentcDNA clones, only 2 were identical in this hypervariable, AU-richregion of the BYV-Cal genome.

Overall, comparison of the Ukrainian and Californian isolates of BYV revealed two large genome regions with very differentlevels of nucleotide sequence similarity. The regions from the5' terminus to the end of ORF 1b (Fig. 1A) were 99.4% identicalbetween the two isolates. In contrast, the 3'-terminal regionsharboring ORFs 2 through 8 had 88.8% identity at the nucleotidelevel.

Identification of BYV genes essential for RNA replication. The mapping of replication-associated functions in the BYV genome was conducted by site-directed mutagenesis of the full-lengthcDNA clone of BYV-Cal (Fig. 1). The roles of the putative RNAhelicase and RNA polymerase domains in genome amplification wereaddressed by introduction of a frameshift mutation (fs in Fig.1A and 2). This mutation introduced the stop codon into ORF 1aupstream from the RNA helicase domain. As expected, Northern hybridizationanalysis of protoplasts harvested at 3.5 days posttransfectiondetected essentially no BYV-specific RNA produced by the fs mutant(Fig. 2A). The input RNA transcripts were most likely degradedby that time. In all subsequent experiments, the fs mutant wasused as a negative control representing a full-size, replication-deficientRNA transcript.

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FIG. 2. Northern hybridization analysis of the plus-strand (A) and minus-strand (B) BYV-specific RNAs in transfected tobacco protoplasts. The RNA transcripts used for protoplast transfections are indicated at the top of each lane. ( $-$ ), no RNA added; WT, wild-type transcript; fs, frameshift mutation in ORF 1a; AN, SB, and SS, expanded deletions in the 3'-terminal part of the BYV genome illustrated in Fig. 1A; g, genomic RNA; int, intermediate-size RNA; numbers, sgRNAs that express corresponding BYV ORFs 2 through 8. The estimated sizes of BYV-Cal sgRNAs are as follows: 2/3, 6.1 kb; 4, 4.4 kb; 5, 2.6 kb; 6, 1.8 kb; 7, 1.2 kb; 8, 0.8 kb (22). The asterisks beside panel B show the positions of background bands.

The possible involvement of products encoded in the 3'-terminal part of the genome in RNA amplification was probed via introductionof a large deletion, AN, into a cDNA clone (Fig. 1A and 2). Thisdeletion removed ORFs 2 through 7 and 55% of ORF 8. The abilityof the AN mutant to accumulate shorter-than-wild-type RNA indicatedthat none of the eight 3'-terminal BYV genes is essential forRNA replication (Fig. 2A and B, lanes WT and AN). However, thelevels of AN RNA accumulation were only 63% ± 11% and 59% ± 15%of the wild-type levels for plus- and minus-strand RNAs, respectively.These results suggested that the deleted region specifies a proteinproduct(s) or RNA element(s) that enhances the accumulation ofBYV RNA in protoplasts.

A second deletion mutant, SB, lacked a region extending from the middle of ORF 3 to nucleotide 15,315, thus reaching intothe 3'-noncoding region (Fig. 1A). The ability of mutant SB toreplicate in protoplasts was completely blocked (Fig. 2A, laneSB), suggesting that the region between the 3'-terminal boundariesof mutants AN and SB (nucleotides 15,061 to 15,315) is requiredfor RNA amplification and is possibly involved in template recognitionby the BYV RNA polymerase.

The third deletion mutant, SS, was also replication deficient (Fig. 2A, lane SS). This result was not unexpected, since thedeletion affected ORF 1b, which encodes the RNA polymerase. The80-amino-acid-long C-terminal region of the RNA polymerase lackingin the SS mutant is conserved among related plant RNA viruses(4). Examination of minus-strand RNA accumulation revealeda pattern similar to that of plus-strand RNAs for all four mutants(Fig. 2B). Since the amount of minus-strand RNA produced duringinfection is lower than that of the plus strands, longer filmexposure resulted in more prominent appearance of the backgroundbands most likely corresponding to plant rRNAs (marked by asterisksin Fig. 2B; reference 14).

Collectively, these experiments indicated that only the products of ORFs 1a and 1b are essential for amplification of BYVRNA, whereas proteins encoded in ORFs 2 to 8 are dispensable forRNA accumulation at the single-cell level.

Requirement of the leader proteinase for efficient RNA amplification. A series of mutations was designed to test if the L-Pro encoded in the 5'-most part of ORF 1a is involved in RNA amplification.Previous analysis revealed that only the papain-like C-terminaldomain of L-Pro, comprising about one-fourth of the molecule,is conserved among closteroviruses (Fig. 3A) (4, 27, 33).Since the remaining about three-fourths of L-Pro exhibited noconserved sequence motifs that could be targeted for mutagenesis,a computer analysis of the protein structure was conducted. Fourstructurally defined regions outside the proteinase domain weretargeted for deletion: a 26-residue-long proline-rich loop inthe 1DL mutant, a 24-residue-long hydrophilic element in the 3DLmutant, and 24- and 32-residue-long amino acid stretches containingshort $alpha$ -helical elements in the 2DL and 4DL mutants (Fig. 3A).The fifth deletion removed nine codons overlapping the L-Pro autocatalyticcleavage site (dcl in Fig. 3). Three larger in-frame deletions,1-B, B-4, and 1-4, removed up to about four-fifths of the variableN-terminal domain of L-Pro (Fig. 3A).

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FIG. 3. Mutagenic analysis of L-Pro function in BYV RNA replication. (A) L-Pro coding region with a summary of the introduced deletions and the BglII site used to generate the 1-B and B-4 mutants. (B) Northern analysis of plus-strand RNA. (C) Northern analysis of minus-strand RNA. 1DL to 4DL, four relatively small (72 to 96 nucleotides) in-frame deletions introduced into the L-Pro-encoding region; dcl, deletion of nine codons, including two glycine codons that specify an L-Pro scissile bond; 1-4, 1-B, and B-4, expanded in-frame deletions in the L-Pro-encoding region outside of the proteinase domain; WT, wild type; fs, frameshift mutation.

It was found that the dcl mutant was replication incompetent (lane dcl in Fig. 3B), suggesting that the cleavage between L-Proand the remainder of the ORF 1a product is essential for genomeamplification. The 2DL, 3DL, and 4DL mutations had relativelymodest effects on RNA accumulation (Fig. 3B and 4), whereas the1DL mutation resulted in over twofold less RNA accumulation. Thelarger deletions 1-B, B-4, and 1-4 resulted in levels of RNA amplificationreaching 20, 57, and 22% of the wild-type level, respectively(Fig. 3B and 4).

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FIG. 4. Effects of the mutations in the L-Pro coding region on the levels of RNA replication and proteolytic activity of L-Pro. The levels of plus or minus strands of genomic RNA in transfected protoplasts were quantified and compared to the level of proteolytic maturation of L-Pro in vitro for each mutant. Values expressed as percentages of the wild type (wt) are means and standard deviations from at least four independent experiments.

The relative effects of L-Pro mutations on minus-strand RNA accumulation were similar to those observed for the plus strands(Fig. 3C and 4). No specific effect on the formation of sgRNAswas revealed (Fig. 3B). These results suggested that L-Pro affectsthe general efficiency of RNA amplification and transcription.

Although all but dcl L-Pro mutations were introduced outside the proteinase domain, the replication defects of the mutantscould be due to the impaired proteolysis. The proteolytic activityof the L-Pro variants was tested in vitro. The RNA transcriptscorresponding to the wild-type and mutant derivatives of the 5'-terminalregion of ORF 1a were translated in wheat germ extracts. It wasrevealed that the dcl mutant directed the formation of the expectedunprocessed ~100-kDa product (data not shown). Approximately 70%of the wild-type translation product was processed in vitro toyield ~66-kDa L-Pro and an ~34-kDa product (not shown). The processingefficiencies of mutants 1DL, 2DL, 3DL, and 1B were not significantlydifferent from that of the wild type (Fig. 4). In contrast, mutants4DL, B-4, and 1-4, in which deletions were located close to theproteinase domain, exhibited markedly lower proteolytic activity(Fig. 4).

However, no direct correlation between processing efficiency and RNA accumulation was found (Fig. 4). This is best exemplifiedby the 1DL and 1-B mutants, in which proteolytic activity wassimilar to that of the wild type, whereas RNA levels were only49 and 19% of the wild-type level, respectively (Fig. 4). Twoconclusions can be drawn from the mutagenic study of the L-Profunction. First, proteolytic processing of the ORF 1a productis strictly required for RNA replication. Second, L-Pro has anadditional function in RNA amplification that is separable fromits proteolytic activity.

Enhancer of RNA accumulation encoded in ORF 8. The replication competence of the AN mutant lacking the 3'-terminal part of the genome indicated that none of ORFs 2 to 8is essential for RNA amplification. However, this large deletionresulted in reduced amplification efficiency, despite the smallersize of the RNA. To test possible roles of ORFs 2 to 8 in replication,point mutations replacing start codons were introduced into eachof these ORFs (Fig. 1A). The levels of RNA accumulation in protoplastswere similar to the wild-type level for all mutant RNA transcriptsbut one (Fig. 5A). The corresponding values were 103% ± 10%, 88%± 17%, 99% ± 9%, 90% ± 10%, 90% ± 24%, 92% ± 11%, and 20% ± 9%for the variants harboring mutations in ORFs 2, 3, 4, 5, 6, 7,and 8, respectively. A fivefold reduction in RNA accumulationobserved for the mutant with the replaced start codon in ORF 8suggested that an important role is played by its product, p21,in RNA amplification (Fig. 5A). Examination of the minus-strandRNA revealed a similar reduction of the RNA level (24% ± 3%; Fig.5B). The levels of sgRNAs were also decreased proportionally,suggesting that p21 has a general stimulating effect on RNA replicationand transcription. Alternatively, p21 could increase RNA levelsby protecting RNA from degradation.

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FIG. 5. Characterization of mutants with replaced start codons in ORFs 2 through 8. (A) Northern analysis of plus-strand RNA. (B) Northern analysis of minus-strand RNA. WT and fs, wild-type and frameshift mutant transcripts used for protoplast transfection, respectively. The numbers at the top correspond to mutant ORFs (cf. Fig. 1A). For designations of BYV-specific and background RNA bands marked by asterisks, see the legend to Fig. 2.

The mutant RNA lacking a start codon in CP-encoding ORF 6 failed to produce an RNA, designated int in Fig. 5A, that migratedbetween genomic RNA and the largest sgRNA. This latter RNA speciesmay be a defective RNA whose formation or stability depends onCP.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Previous comparative analysis of the BYV and CTV genomes revealed that proteins encoded by ORFs 1a and 1b possess conserveddomains characteristic of the replicases of Sindbis virus-likeviruses (4, 17, 27). In contrast to the single-componentgenomes of BYV and CTV, the genome of lettuce infectious yellowsclosterovirus is divided among two RNAs (33). RNA 1 harborsORFs 1a and 1b and an additional ORF that is unique to lettuceinfectious yellows closterovirus. RNA 2 codes for homologs ofBYV p6, HSP70h, p64, CP, CPm, and a protein with marginal similarityto p21 (33). It was demonstrated recently that RNA 1 can replicatein the absence of RNA 2 but not vice versa (34). This resultfurther supported the involvement of the products of ORFs 1a and1b in RNA replication, while the possible roles of several additionalproteins encoded in one- or two-component closteroviruses remainedelusive.

Generation of a full-length BYV clone permitted mapping of the genes involved in the replication and transcription of the15.5-kb viral RNA. As expected, expression of intact ORFs 1a and1b, encoding putative methyltransferase, RNA helicase, and RNApolymerase, was found to be essential for RNA replication. Deletionof the cleavage site located between L-Pro and the rest of theORF 1a product abolished RNA replication, suggesting that autocatalyticrelease of L-Pro or maintenance of a proper protein structurearound the cleavage site is critical for virus viability. In additionto the conserved papain-like proteinase domain, closterovirusL-Pro possesses a variable N-terminal domain (4, 27, 33).A function of this domain was probed by using a series of deletionmutants. Analysis of the mutant phenotypes revealed that the N-terminaldomain is required for efficient amplification of the BYV genome.This function was separable from proteinase activity, since somemutants that exhibited no detectable processing defects accumulatedreduced levels of RNA. The ability of an L-Pro mutant lackingmost of the N-terminal domain to replicate, albeit inefficiently,suggested that the function of this domain in genome amplificationis accessory rather than essential.

The possibility cannot be excluded that at least some of the deletions in the L-Pro-encoding region disturbed the RNA elements(e.g., RNA polymerase recognition signals) that are directly involvedin the RNA accumulation process. These elements, however, arenormally distinct for the plus and minus RNA strands. Since analyzedL-Pro mutations affected the accumulation of both strands to similarextents, it seems more likely that the observed effects were mediatedby encoded protein products rather than by the RNA itself.

Interestingly, mutational analysis of the helper component proteinase (HC-Pro) encoded in plant potyviruses revealed a similarfunctional profile. Processing activity of the C-terminal papain-likeproteinase domain of HC-Pro (8) was found to be indispensablefor RNA replication (30), whereas the central domain functionedas a replicational enhancer (6, 31). Recent experiments suggestedthat HC-Pro activates RNA synthesis indirectly, possibly disarmingthe host defense system that limits the accumulation of viralRNA (31, 46).

Both potyvirus HC-Pro and closterovirus L-Pro belong to a large class of papain-like leader proteinases that provide variousaccessory functions in viral reproduction (19, 21). Additionalexamples include the aphthovirus L-proteinase that is involvedin the shutoff of host protein synthesis and in virus pathogenicity(43, 45) and p29, a symptom determinant of the hypovirulence-associatedvirus of chestnut blight fungus (10). It appears that diverseplant, animal, and fungal viruses recruit papain-like proteinasesto manipulate host functions in the course of an infection.

Six genes located in the 3'-terminal region of the BYV genome were found to be dispensable for virus RNA accumulation at thesingle-cell level. It seems likely that corresponding productsp6, HSP70h, p64, CPm, CP, and p20 contribute to the processesof virion assembly, cell-to-cell and long-distance transport,and aphid transmission of BYV. On the other hand, p21, encodedby the 3'-most BYV gene, was identified as an enhancer of RNAamplification. The mutant lacking the p21 start codon exhibiteda fivefold reduction in the accumulation of both the plus andminus strands of genomic RNA. The proteins related to p21 areconserved in other one-component closteroviruses, such as CTVand beet yellow stunt virus (17, 28, and data not shown).Although a database search did not reveal any non-closterovirushomologs of p21, the $gamma$ b protein encoded in barley stripe mosaichordeivirus seems to perform an analogous accessory function inRNA replication (44). It should be emphasized that none of themutations in p21, in L-Pro, or in products of ORFs 2 through 7specifically affected the synthesis of sgRNAs. These data suggestthat the only closterovirus proteins required for genome transcriptionare the products of ORFs 1a and 1b.

Interesting analogies were observed in the organization and expression of closterovirus and coronavirus genomes (17). Theseanalogies included unusually large replicases encoded in ORFs1a and 1b, with ORF 1b expressed via translational frameshift;the presence of papain-like proteinases in the 5'-proximal partof ORF 1a; and the formation of multiple sgRNAs required for expressionof non-replicase genes (11, 21, 37, 38). The functionalanalysis presented here revealed that closteroviruses, similarto coronavirus-like viruses (32), in addition to replicase,do require a product of the 3'-most ORF for efficient RNA amplification.Further mechanistic studies employing full-length cDNA clonesof coronavirus-like viruses (49) and closteroviruses shouldexplain why these two phylogenetically and biologically diversevirus groups convergently adopted this particular combinationof genome replication and expression strategies in the courseof evolution towards the largest known "RNA chromosomes."

	ACKNOWLEDGMENTS

We thank William Dawson, Theo Dreher, Bryce Falk, Alexander Karasev, Eugene Koonin, and Arcady Mushegian for helpful discussionsand Theo Dreher and William Dawson for critical reading of themanuscript.

This work was supported by a James A. Shannon Director's Award from the National Institute of General Medical Sciences, NationalInstitutes of Health (R5GM53190A), and by a grant from the NationalResearch Initiative Competitive Grants Program of the U.S. Departmentof Agriculture (97-35303-4515).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Botany and Plant Pathology, Oregon State University, Cordley Hall 2082,Corvallis, OR 97331. Phone: (541) 737-5472. Fax: (541) 737-3573.E-mail: doljav{at}bcc.orst.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Adkins, S., R. W. Siegel, J. H. Sun, and C. C. Kao. 1997. Minimal templates directing accurate initiation of subgenomic RNA synthesis in vitro by the brome mosaic virus RNA-dependent RNA polymerase. RNA 3:634-647[Abstract].

2. Agranovsky, A. A., V. P. Boyko, A. V. Karasev, E. V. Koonin, and V. V. Dolja. 1991. Putative 65kDa protein of beet yellows closterovirus is a homologue of HSP70 heat shock proteins. J. Mol. Biol. 217:603-610[Medline].

3. Agranovsky, A. A., V. P. Boyko, A. V. Karasev, N. A. Lunina, E. V. Koonin, and V. V. Dolja. 1991. Nucleotide sequence of the 3'-terminal half of beet yellows closterovirus RNA genome: unique arrangement of eight virus genes. J. Gen. Virol. 72:15-23[Abstract/Free Full Text].

4. Agranovsky, A. A., E. V. Koonin, V. P. Boyko, E. Maiss, R. Frotschl, N. A. Lunina, and J. G. Atabekov. 1994. Beet yellows closterovirus: complete genome structure and identification of a leader papain-like thiol protease. Virology 198:311-324[Medline].

5. Agranovsky, A. A., D. E. Lesemann, E. Maiss, R. Hull, and J. G. Atabekov. 1995. "Rattlesnake" structure of a filamentous plant RNA virus built of two capsid proteins. Proc. Natl. Acad. Sci. USA 92:2470-2473[Abstract/Free Full Text].

6. Atreya, C. D., and T. P. Pirone. 1993. Mutational analysis of the helper component-proteinase gene of a potyvirus: effects of amino acid substitutions, deletions, and gene replacement on virulence and aphid transmissibility. Proc. Natl. Acad. Sci. USA 90:11919-11923[Abstract/Free Full Text].

6a. Bio-Rad Laboratories. 1987. In Bio-Rad bulletin 1393. Bio-Rad Laboratories, Richmond, Calif.

7. Boyko, V. P., A. V. Karasev, A. A. Agranovsky, E. V. Koonin, and V. V. Dolja. 1992. Capsid protein gene duplication in a filamentous RNA virus of plants. Proc. Natl. Acad. Sci. USA 89:9156-9160[Abstract/Free Full Text].

8. Carrington, J. C., S. M. Cary, T. D. Parks, and W. G. Dougherty. 1989. A second proteinase encoded by a plant potyvirus genome. EMBO J. 8:365-370[Medline].

9. Collmer, C. W., and J. M. Kaper. 1985. Double-stranded RNAs of cucumber mosaic virus and its satellite contain an unpaired terminal guanosine: implications for replication. Virology 145:249-259[Medline].

10. Craven, M. G., D. M. Pawlyk, G. H. Choi, and D. L. Nuss. 1993. Papain-like protease p29 as a symptom determinant encoded by a hypovirulence-associated virus of the chestnut blight fungus. J. Virol. 67:6513-6521[Abstract/Free Full Text].

11. den Boon, J. A., K. S. Faaberg, J. J. M. Meulenberg, A. L. M. Wassenaar, P. G. W. Plagemann, A. E. Gorbalenya, and E. J. Snijder. 1995. Processing and evolution of the N-terminal region of the arterivirus replicase ORF1a protein: identification of two papainlike cysteine proteases. J. Virol. 69:4500-4505[Abstract].

12. Dolja, V. V., and J. G. Atabekov. 1987. The structure of barley stripe mosaic double-stranded RNAs. FEBS Lett. 214:313-316.

13. Dolja, V. V., D. P. Grama, S. Y. Morozov, and J. G. Atabekov. 1987. Potato virus X-related single- and double-stranded RNAs: characterization and identification of terminal structures. FEBS Lett. 214:308-312.

14. Dolja, V. V., A. V. Karasev, and A. A. Agranovsky. 1990. Organization of beet yellows closterovirus genome, p. 31-35. In R. Rueckert, and M. Brinton (ed.), New aspects of positive-strand RNA viruses. ASM Press, Washington, D.C.

15. Dolja, V. V., H. J. McBride, and J. C. Carrington. 1992. Tagging of plant potyvirus replication and movement by insertion of $beta$ -glucuronidase (GUS) into the viral polyprotein. Proc. Natl. Acad. Sci. USA 89:10208-10212[Abstract/Free Full Text].

16. Dolja, V. V., K. L. Herndon, T. P. Pirone, and J. C. Carrington. 1993. Spontaneous mutagenesis of a plant potyvirus genome after insertion of a foreign gene. J. Virol. 67:5968-5975[Abstract/Free Full Text].

17. Dolja, V. V., A. V. Karasev, and E. V. Koonin. 1994. Molecular biology and evolution of closteroviruses: sophisticated build-up of large RNA genomes. Annu. Rev. Phytopathol. 32:261-285.

18. Dolja, V. V., J. Hong, K. E. Keller, R. R. Martin, and V. V. Peremyslov. 1997. Suppression of potyvirus infection by coexpressed closterovirus protein. Virology 234:243-252[Medline].

19. Dougherty, W. G., and B. L. Semler. 1993. Expression of virus-encoded proteinases: functional and structural similarities with cellular enzymes. Microbiol. Rev. 57:781-822[Abstract/Free Full Text].

20. French, R., and P. Ahlquist. 1988. Characterization and engineering of sequences controlling in vivo synthesis of brome mosaic virus subgenomic RNA. J. Virol. 62:2411-2420[Abstract/Free Full Text].

21. Gorbalenya, A. E., E. V. Koonin, and M. M.-C. Lai. 1991. Putative papain-related thiol proteases of positive-strand RNA viruses. FEBS Lett. 288:201-205[Medline].

22. He, X.-H., A. L. N. Rao, and R. Creamer. 1997. Characterization of beet yellows closterovirus-specific RNAs in infected plants and protoplasts. Phytopathology 87:347-352[Medline].

23. Herz, J. M., and H. V. Huang. 1995. Evolution of the Sindbis virus subgenomic mRNA promoter in cultured cells. J. Virol. 69:7768-7774[Abstract].

24. Hilf, M. E., A. V. Karasev, H. R. Pappu, D. J. Gumpf, C. L. Niblett, and S. M. Garnsey. 1995. Characterization of citrus tristeza virus subgenomic RNAs in infected tissue. Virology 208:576-582[Medline].

25. Jeong, Y. S., and S. Makino. 1994. Evidence for coronavirus discontinuous transcription. J. Virol. 68:2615-2623[Abstract/Free Full Text].

26. Karasev, A. V., A. A. Agranovsky, V. V. Rogov, N. A. Miroshnichenko, V. V. Dolja, and J. G. Atabekov. 1989. Virion RNA of beet yellows closterovirus: cell-free translation and some properties. J. Gen. Virol. 70:241-245.

27. Karasev, A. V., V. P. Boyko, S. Gowda, O. V. Nikolaeva, M. E. Hilf, E. V. Koonin, C. L. Niblett, K. Cline, D. J. Gumpf, R. F. Lee, S. M. Garnsey, D. J. Lewandowski, and W. O. Dawson. 1995. Complete sequence of the citrus tristeza virus RNA genome. Virology 208:511-520[Medline].

28. Karasev, A. V., O. V. Nikolaeva, A. R. Mushegian, R. F. Lee, and W. O. Dawson. 1996. Organization of the 3'-terminal half of beet yellow stunt virus genome and implications for the evolution of closteroviruses. Virology 221:199-207[Medline].

29. Karasev, A. V., M. E. Hilf, S. M. Garnsey, and W. O. Dawson. 1997. Transcriptional strategy of closteroviruses: mapping the 5' termini of the citrus tristeza virus subgenomic RNAs. J. Virol. 71:6233-6236[Abstract].

30. Kasschau, K. D., and J. C. Carrington. 1995. Requirement for HC-Pro during genome amplification of tobacco etch potyvirus. Virology 209:268-273[Medline].

31. Kasschau, K. D., S. Cronin, and J. C. Carrington. 1997. Genome amplification and long-distance movement functions associated with the central domain of tobacco etch potyvirus helper component-proteinase. Virology 228:251-262[Medline].

32. Kim, K. H., and S. Makino. 1995. Two murine coronavirus genes suffice for viral RNA synthesis. J. Virol. 69:2313-2321[Abstract].

33. Klaassen, V. A., M. Boeshore, E. V. Koonin, T. Tian, and B. W. Falk. 1995. Genome structure and phylogenetic analysis of lettuce infectious yellows virus, a whitefly transmitted, bipartite closterovirus. Virology 208:99-110[Medline].

34. Klaassen, V. A., D. Mayhew, D. Fisher, and B. W. Falk. 1996. In vitro transcripts from cloned cDNAs of the lettuce infectious yellows closterovirus bipartite genomic RNAs are competent for replication in Nicotiana benthamiana protoplasts. Virology 222:169-175[Medline].

35. Koonin, E. V., and V. V. Dolja. 1993. Evolution and taxonomy of positive-strand RNA viruses: implications of comparative analysis of amino acid sequences. Crit. Rev. Biochem. Mol. Biol. 28:375-430[Medline].

36. Kunkel, T. A., J. D. Roberts, and R. Zakour. 1987. Rapid and efficient site-specific mutagenesis without phenotypic selection. Methods Enzymol. 154:367-382[Medline].

37. Lai, M. M. C. 1990. Coronavirus: organization, replication, and expression of genome. Annu. Rev. Microbiol. 44:303-333[Medline].

38. Lai, M. M. C. 1997. RNA-protein interactions in the regulation of coronavirus RNA replication and transcription. Biol. Chem. 378:477-481. [Medline]

39. Levis, R., S. Schlesinger, and H. V. Huang. 1990. Promoter for Sindbis virus RNA-dependent subgenomic RNA transcription. J. Virol. 64:1726-1733[Abstract/Free Full Text].

40. Marsh, L. E., T. W. Dreher, and T. C. Hall. 1988. Mutational analysis of the core and modulator sequences of the BMV RNA3 subgenomic promoter. Nucleic Acids Res. 16:981-995[Abstract/Free Full Text].

41. Navas-Castillo, J., M. R. Albiach-Marti, S. Gowda, M. Hilf, S. M. Garnsey, and W. O. Dawson. 1997. Kinetics of accumulation of citrus tristeza virus RNAs in host and non-host protoplasts. Virology 228:92-97[Medline].

42. Oh, C.-S., and J. C. Carrington. 1989. Identification of essential residues in potyvirus proteinase HC-Pro by site-directed mutagenesis. Virology 173:692-699[Medline].

43. Ohlmann, T., V. M. Pain, W. Wood, M. Rau, and S. J. Morley. 1997. The proteolytic cleavage of eukaryotic initiation factor (eIF) 4G is prevented by eIF4E binding protein (PHAS-I; 4E-BP1) in the reticulocyte lysate. EMBO J. 16:844-855[Medline].

44. Petty, I. T. D., R. French, R. W. Jones, and A. O. Jackson. 1990. Identification of barley stripe mosaic virus genes involved in viral RNA replication and systemic movement. EMBO J. 9:3453-3457[Medline].

45. Piccone, M. E., E. Rieder, P. W. Mason, and M. J. Grubman. 1995. The foot-and-mouth disease virus leader proteinase gene is not required for viral replication. J. Virol. 69:5376-5382[Abstract].

46. Pruss, G., X. Ge, X. M. Shi, J. C. Carrington, and V. B. Vance. 1997. Plant viral synergism: the potyviral genome encodes a broad-range pathogenicity enhancer that transactivates replication of heterologous viruses. Plant Cell 9:859-868[Abstract/Free Full Text].

47. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. In Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.

48. Valverde, R. A., S. T. Nameth, and R. L. Jordan. 1990. Analysis of double-stranded RNA for plant virus diagnosis. Plant Dis. 74:255-258.

49. van Dinten, L. C., J. A. den Boon, A. L. M. Wassenaar, W. J. M. Spaan, and E. J. Snijder. 1997. An infectious arterivirus cDNA clone: identification of a replicase point mutation that abolishes discontinuous mRNA transcription. Proc. Natl. Acad. Sci. USA 94:991-996[Abstract/Free Full Text].

50. van Marle, G., W. Luytjes, R. van der Most, T. van der Straaten, and W. J. Spaan. 1995. Regulation of coronavirus mRNA transcription. J. Virol. 69:7851-7856[Abstract].

51. Zhang, X., C.-L. Liao, and M. M. C. Lai. 1994. Coronavirus leader RNA regulates and initiates subgenomic RNA transcription both in trans and in cis. J. Virol. 68:4738-4746[Abstract/Free Full Text].

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1.	Adkins, S., R. W. Siegel, J. H. Sun, and C. C. Kao. 1997. Minimal templates directing accurate initiation of subgenomic RNA synthesis in vitro by the brome mosaic virus RNA-dependent RNA polymerase. RNA 3:634-647[Abstract].
2.	Agranovsky, A. A., V. P. Boyko, A. V. Karasev, E. V. Koonin, and V. V. Dolja. 1991. Putative 65kDa protein of beet yellows closterovirus is a homologue of HSP70 heat shock proteins. J. Mol. Biol. 217:603-610[Medline].
3.	Agranovsky, A. A., V. P. Boyko, A. V. Karasev, N. A. Lunina, E. V. Koonin, and V. V. Dolja. 1991. Nucleotide sequence of the 3'-terminal half of beet yellows closterovirus RNA genome: unique arrangement of eight virus genes. J. Gen. Virol. 72:15-23[Abstract/Free Full Text].
4.	Agranovsky, A. A., E. V. Koonin, V. P. Boyko, E. Maiss, R. Frotschl, N. A. Lunina, and J. G. Atabekov. 1994. Beet yellows closterovirus: complete genome structure and identification of a leader papain-like thiol protease. Virology 198:311-324[Medline].
5.	Agranovsky, A. A., D. E. Lesemann, E. Maiss, R. Hull, and J. G. Atabekov. 1995. "Rattlesnake" structure of a filamentous plant RNA virus built of two capsid proteins. Proc. Natl. Acad. Sci. USA 92:2470-2473[Abstract/Free Full Text].
6.	Atreya, C. D., and T. P. Pirone. 1993. Mutational analysis of the helper component-proteinase gene of a potyvirus: effects of amino acid substitutions, deletions, and gene replacement on virulence and aphid transmissibility. Proc. Natl. Acad. Sci. USA 90:11919-11923[Abstract/Free Full Text].
6a.	Bio-Rad Laboratories. 1987. In Bio-Rad bulletin 1393. Bio-Rad Laboratories, Richmond, Calif.
7.	Boyko, V. P., A. V. Karasev, A. A. Agranovsky, E. V. Koonin, and V. V. Dolja. 1992. Capsid protein gene duplication in a filamentous RNA virus of plants. Proc. Natl. Acad. Sci. USA 89:9156-9160[Abstract/Free Full Text].
8.	Carrington, J. C., S. M. Cary, T. D. Parks, and W. G. Dougherty. 1989. A second proteinase encoded by a plant potyvirus genome. EMBO J. 8:365-370[Medline].
9.	Collmer, C. W., and J. M. Kaper. 1985. Double-stranded RNAs of cucumber mosaic virus and its satellite contain an unpaired terminal guanosine: implications for replication. Virology 145:249-259[Medline].
10.	Craven, M. G., D. M. Pawlyk, G. H. Choi, and D. L. Nuss. 1993. Papain-like protease p29 as a symptom determinant encoded by a hypovirulence-associated virus of the chestnut blight fungus. J. Virol. 67:6513-6521[Abstract/Free Full Text].
11.	den Boon, J. A., K. S. Faaberg, J. J. M. Meulenberg, A. L. M. Wassenaar, P. G. W. Plagemann, A. E. Gorbalenya, and E. J. Snijder. 1995. Processing and evolution of the N-terminal region of the arterivirus replicase ORF1a protein: identification of two papainlike cysteine proteases. J. Virol. 69:4500-4505[Abstract].
12.	Dolja, V. V., and J. G. Atabekov. 1987. The structure of barley stripe mosaic double-stranded RNAs. FEBS Lett. 214:313-316.
13.	Dolja, V. V., D. P. Grama, S. Y. Morozov, and J. G. Atabekov. 1987. Potato virus X-related single- and double-stranded RNAs: characterization and identification of terminal structures. FEBS Lett. 214:308-312.
14.	Dolja, V. V., A. V. Karasev, and A. A. Agranovsky. 1990. Organization of beet yellows closterovirus genome, p. 31-35. In R. Rueckert, and M. Brinton (ed.), New aspects of positive-strand RNA viruses. ASM Press, Washington, D.C.
15.	Dolja, V. V., H. J. McBride, and J. C. Carrington. 1992. Tagging of plant potyvirus replication and movement by insertion of $beta$ -glucuronidase (GUS) into the viral polyprotein. Proc. Natl. Acad. Sci. USA 89:10208-10212[Abstract/Free Full Text].
16.	Dolja, V. V., K. L. Herndon, T. P. Pirone, and J. C. Carrington. 1993. Spontaneous mutagenesis of a plant potyvirus genome after insertion of a foreign gene. J. Virol. 67:5968-5975[Abstract/Free Full Text].
17.	Dolja, V. V., A. V. Karasev, and E. V. Koonin. 1994. Molecular biology and evolution of closteroviruses: sophisticated build-up of large RNA genomes. Annu. Rev. Phytopathol. 32:261-285.
18.	Dolja, V. V., J. Hong, K. E. Keller, R. R. Martin, and V. V. Peremyslov. 1997. Suppression of potyvirus infection by coexpressed closterovirus protein. Virology 234:243-252[Medline].
19.	Dougherty, W. G., and B. L. Semler. 1993. Expression of virus-encoded proteinases: functional and structural similarities with cellular enzymes. Microbiol. Rev. 57:781-822[Abstract/Free Full Text].
20.	French, R., and P. Ahlquist. 1988. Characterization and engineering of sequences controlling in vivo synthesis of brome mosaic virus subgenomic RNA. J. Virol. 62:2411-2420[Abstract/Free Full Text].
21.	Gorbalenya, A. E., E. V. Koonin, and M. M.-C. Lai. 1991. Putative papain-related thiol proteases of positive-strand RNA viruses. FEBS Lett. 288:201-205[Medline].
22.	He, X.-H., A. L. N. Rao, and R. Creamer. 1997. Characterization of beet yellows closterovirus-specific RNAs in infected plants and protoplasts. Phytopathology 87:347-352[Medline].
23.	Herz, J. M., and H. V. Huang. 1995. Evolution of the Sindbis virus subgenomic mRNA promoter in cultured cells. J. Virol. 69:7768-7774[Abstract].
24.	Hilf, M. E., A. V. Karasev, H. R. Pappu, D. J. Gumpf, C. L. Niblett, and S. M. Garnsey. 1995. Characterization of citrus tristeza virus subgenomic RNAs in infected tissue. Virology 208:576-582[Medline].
25.	Jeong, Y. S., and S. Makino. 1994. Evidence for coronavirus discontinuous transcription. J. Virol. 68:2615-2623[Abstract/Free Full Text].
26.	Karasev, A. V., A. A. Agranovsky, V. V. Rogov, N. A. Miroshnichenko, V. V. Dolja, and J. G. Atabekov. 1989. Virion RNA of beet yellows closterovirus: cell-free translation and some properties. J. Gen. Virol. 70:241-245.
27.	Karasev, A. V., V. P. Boyko, S. Gowda, O. V. Nikolaeva, M. E. Hilf, E. V. Koonin, C. L. Niblett, K. Cline, D. J. Gumpf, R. F. Lee, S. M. Garnsey, D. J. Lewandowski, and W. O. Dawson. 1995. Complete sequence of the citrus tristeza virus RNA genome. Virology 208:511-520[Medline].
28.	Karasev, A. V., O. V. Nikolaeva, A. R. Mushegian, R. F. Lee, and W. O. Dawson. 1996. Organization of the 3'-terminal half of beet yellow stunt virus genome and implications for the evolution of closteroviruses. Virology 221:199-207[Medline].
29.	Karasev, A. V., M. E. Hilf, S. M. Garnsey, and W. O. Dawson. 1997. Transcriptional strategy of closteroviruses: mapping the 5' termini of the citrus tristeza virus subgenomic RNAs. J. Virol. 71:6233-6236[Abstract].
30.	Kasschau, K. D., and J. C. Carrington. 1995. Requirement for HC-Pro during genome amplification of tobacco etch potyvirus. Virology 209:268-273[Medline].
31.	Kasschau, K. D., S. Cronin, and J. C. Carrington. 1997. Genome amplification and long-distance movement functions associated with the central domain of tobacco etch potyvirus helper component-proteinase. Virology 228:251-262[Medline].
32.	Kim, K. H., and S. Makino. 1995. Two murine coronavirus genes suffice for viral RNA synthesis. J. Virol. 69:2313-2321[Abstract].
33.	Klaassen, V. A., M. Boeshore, E. V. Koonin, T. Tian, and B. W. Falk. 1995. Genome structure and phylogenetic analysis of lettuce infectious yellows virus, a whitefly transmitted, bipartite closterovirus. Virology 208:99-110[Medline].
34.	Klaassen, V. A., D. Mayhew, D. Fisher, and B. W. Falk. 1996. In vitro transcripts from cloned cDNAs of the lettuce infectious yellows closterovirus bipartite genomic RNAs are competent for replication in Nicotiana benthamiana protoplasts. Virology 222:169-175[Medline].
35.	Koonin, E. V., and V. V. Dolja. 1993. Evolution and taxonomy of positive-strand RNA viruses: implications of comparative analysis of amino acid sequences. Crit. Rev. Biochem. Mol. Biol. 28:375-430[Medline].
36.	Kunkel, T. A., J. D. Roberts, and R. Zakour. 1987. Rapid and efficient site-specific mutagenesis without phenotypic selection. Methods Enzymol. 154:367-382[Medline].
37.	Lai, M. M. C. 1990. Coronavirus: organization, replication, and expression of genome. Annu. Rev. Microbiol. 44:303-333[Medline].
38.	Lai, M. M. C. 1997. RNA-protein interactions in the regulation of coronavirus RNA replication and transcription. Biol. Chem. 378:477-481. [Medline]
39.	Levis, R., S. Schlesinger, and H. V. Huang. 1990. Promoter for Sindbis virus RNA-dependent subgenomic RNA transcription. J. Virol. 64:1726-1733[Abstract/Free Full Text].
40.	Marsh, L. E., T. W. Dreher, and T. C. Hall. 1988. Mutational analysis of the core and modulator sequences of the BMV RNA3 subgenomic promoter. Nucleic Acids Res. 16:981-995[Abstract/Free Full Text].
41.	Navas-Castillo, J., M. R. Albiach-Marti, S. Gowda, M. Hilf, S. M. Garnsey, and W. O. Dawson. 1997. Kinetics of accumulation of citrus tristeza virus RNAs in host and non-host protoplasts. Virology 228:92-97[Medline].
42.	Oh, C.-S., and J. C. Carrington. 1989. Identification of essential residues in potyvirus proteinase HC-Pro by site-directed mutagenesis. Virology 173:692-699[Medline].
43.	Ohlmann, T., V. M. Pain, W. Wood, M. Rau, and S. J. Morley. 1997. The proteolytic cleavage of eukaryotic initiation factor (eIF) 4G is prevented by eIF4E binding protein (PHAS-I; 4E-BP1) in the reticulocyte lysate. EMBO J. 16:844-855[Medline].
44.	Petty, I. T. D., R. French, R. W. Jones, and A. O. Jackson. 1990. Identification of barley stripe mosaic virus genes involved in viral RNA replication and systemic movement. EMBO J. 9:3453-3457[Medline].
45.	Piccone, M. E., E. Rieder, P. W. Mason, and M. J. Grubman. 1995. The foot-and-mouth disease virus leader proteinase gene is not required for viral replication. J. Virol. 69:5376-5382[Abstract].
46.	Pruss, G., X. Ge, X. M. Shi, J. C. Carrington, and V. B. Vance. 1997. Plant viral synergism: the potyviral genome encodes a broad-range pathogenicity enhancer that transactivates replication of heterologous viruses. Plant Cell 9:859-868[Abstract/Free Full Text].
47.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. In Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
48.	Valverde, R. A., S. T. Nameth, and R. L. Jordan. 1990. Analysis of double-stranded RNA for plant virus diagnosis. Plant Dis. 74:255-258.
49.	van Dinten, L. C., J. A. den Boon, A. L. M. Wassenaar, W. J. M. Spaan, and E. J. Snijder. 1997. An infectious arterivirus cDNA clone: identification of a replicase point mutation that abolishes discontinuous mRNA transcription. Proc. Natl. Acad. Sci. USA 94:991-996[Abstract/Free Full Text].
50.	van Marle, G., W. Luytjes, R. van der Most, T. van der Straaten, and W. J. Spaan. 1995. Regulation of coronavirus mRNA transcription. J. Virol. 69:7851-7856[Abstract].
51.	Zhang, X., C.-L. Liao, and M. M. C. Lai. 1994. Coronavirus leader RNA regulates and initiates subgenomic RNA transcription both in trans and in cis. J. Virol. 68:4738-4746[Abstract/Free Full Text].