Uncoupled Expression of p33 and p92 Permits Amplification of Tomato Bushy Stunt Virus RNAs

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J Virol, July 1998, p. 5845-5851, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Uncoupled Expression of p33 and p92 Permits Amplification of Tomato Bushy Stunt Virus RNAs

Sara K. Oster, Baodong Wu, and K. Andrew White^*

Department of Biology, York University, Toronto, Ontario, Canada M3J 1P3

Received 5 February 1998/Accepted 25 March 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Tomato bushy stunt virus (TBSV) is a plus-sense RNA virus which encodes a 33-kDa protein in its 5'-most open reading frame(ORF). Readthrough of the amber stop codon of the p33 ORF resultsin the production of a 92-kDa fusion protein. Both of these productsare expressed directly from the viral genome and are suspectedto be involved in viral RNA replication. We have investigatedfurther the roles of these proteins in the amplification of viralRNAs by using a complementation system in which p33 and p92 areexpressed from different viral RNAs. Our results indicate that(i) both of these proteins are necessary for viral RNA amplification;(ii) translation of these proteins can be uncoupled while maintainingamplification of viral RNAs; (iii) if compatibility requirementsexist between p33 and p92, they are not exceptionally strict;and (iv) the C-terminal ~6% of p33 is necessary for its functionalactivity. Interestingly, no complementation was observed whena p33-encoding replicon containing a deletion of a 3'-locatedsegment, region 3.5, was tested. However, when 5'-capped transcriptsof the same replicon were analyzed, complementation allowing forRNA amplification was observed. This ability to compensate functionallyfor the absence of region 3.5 by the addition of a 5' cap suggeststhat this RNA segment may act as a translational enhancer forthe expression of virally encoded products.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Plant RNA viruses have various genome organizations and use a wide array of gene expression strategies (4, 14, 30).Despite such differences, these viruses are unified by the factthat they all encode components of an RNA-dependent RNA polymeraseactivity involved in the replication of their genomes. Conservedmotifs have been identified within these viral proteins, whichhave been implicated in specific functions in genome replicationsuch as polymerase, helicase, and/or RNA-capping activities (5,12, 17). These activities may be combined on a single proteinor divided among two or more products, which, in turn, may beencoded in different RNA segments in multipartite genomes (30).

A common strategy used by several RNA plant virus genera (including Tobamovirus, Furovirus, Tobravirus, Necrovirus, Tombusvirus,and Carmovirus) is to encode their two protein replication componentsin the 5'-most open reading frame (ORF) and in a readthrough productof that ORF (30). Both of these products are translated directlyfrom the viral genome, but the amount of readthrough product isgenerally orders of magnitude lower than that of the prereadthroughproduct (13, 22, 29), due to relatively inefficient suppressionof the termination codon (23, 24). For tobacco mosaic virus,the 183-kDa readthrough product alone is sufficient for viralRNA replication but the viral RNA accumulation levels are significantlyreduced compared to when both the pre- and readthrough productsare present (7). This is in contrast to the Carmovirus turnipcrinkle virus (TCV), where both the p28 prereadthrough and p88readthrough products are required (29). For members of the genusTombusvirus (1, 6, 16, 18, 25), there is some evidencesuggesting a similar requirement for both products (1, 22).

The genome of tomato bushy stunt virus (TBSV, the prototype of the genus Tombusvirus) is a monopartite, positive-sense RNAof 4.7 kb (6). It is not polyadenylated, and it contains fivefunctional ORFs (Fig. 1) (6). The genome is not thought tobe 5' capped, since that of the closely related carnation Italianringspot Tombusvirus has been shown not to contain such a structure(18). The 5'-most ORF in the TBSV genome encodes a 33-kDa protein,which has been proposed to function in viral RNA replication (22);however, its amino acid sequence does not contain any known motifsthat would define it as such. Readthrough of the amber stop codonof the p33 ORF results in the translation of a 92-kDa fusion protein,the readthrough portion of which contains highly conserved motifsfound in catalytic subunits of RNA-dependent RNA polymerases (6,12). The coat protein, a 41-kDa product, is encoded by ORF3,and the p22 and p19 movement/symptom-related products are encodedby the two 3'-most ORFs, which overlap in different reading frames(20, 21). The products of ORF3 through ORF5 are translatedfrom two subgenomic (sg) mRNAs, which are synthesized during infections(6).

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FIG. 1. Schematic representation of TBSV genome and various defective viral RNAs. The wt TBSV genome (T-100) is shown at the top as a thick horizontal line, with coding regions depicted as boxes which include the approximate molecular weights (in thousands) of the encoded proteins (6). The translation product p33 and its readthrough product p92 are indicated as arrows below the genome, and the approximate position of region 3.5 is shown as a small black box near the 3' end of the genome. HS-175 is a mutant of the genome in which the p33 termination codon has been replaced by a tyrosine codon to allow the expression of p92 (arrow) but not p33 (22). Various smaller defective viral RNAs are depicted in which shaded boxes correspond to regions of the genome retained in these molecules whereas thin horizontal lines correspond to genomic segments which are absent. DI-82 and DI-83 both encode p33 (open box) and are identical, except that region 3.5 is deleted from DI-82 (28). DI-83 $Delta$ MfeI is structurally similar to DI-83 but encodes a C-terminally truncated form of p33 (open box), which contains a C-terminal extension of 18 aa from a different reading frame (adjoining black box). DI-72 and DI-73 are composed of four and three noncontiguous regions, respectively (i.e., regions I through IV and I through III/IV, respectively), encode no functional proteins, and are identical except that region 3.5 is absent in DI-72 (28).

The TBSV p33 and p92 products are translated directly from the genome, and the ratio of their accumulation levels in vivohas been estimated at 20:1 (22). The precise efficiency of readthroughof the amber stop codon of p33 in TBSV is unknown, but in anothermember of the family Tombusviridae (i.e., TCV), readthrough occursin vivo with an efficiency of approximately 1% (29). It is unclearhow efficient translation of the p33 product (and to a lesserextent p92) is accomplished, since the TBSV genome does not appearto contain structures known to enhance translation in eukaryoticcells [i.e., a 5' cap structure and a 3' poly(A) tail]. It ispossible, therefore, that the genome contains other structureswhose role is to enhance translation; however, such elements havenot yet been identified. A nonconventional translational enhancerelement has been described in barley yellow dwarf virus (BYDV-PAV)(26). BYDV-PAV is a Luteovirus (subgroup I) which contains aplus-strand RNA genome which lacks a 5' cap structure and poly(A)tail. Similar to the other viral genomes discussed, BYDV-PAV encodestwo RNA replication-related products at the 5' end of its genome;however, its corresponding fusion product is generated via a $-$ 1frameshift mechanism rather than by readthrough (15). Basedon amino acid comparisons of virus-encoded polymerase components,tombusviruses and luteoviruses (subgroup I) are related and havebeen assigned to the same supergroup of viruses (supergroup II)(3). Wang et al. (26) have shown that for BYDV-PAV the expressionof the 5' ORF is stimulated by an RNA segment located near the3' terminus. This stimulatory activity was lost when mutationswere introduced into this 3'-translational enhancer (3'TE), butefficient translation was recovered by the addition of a 5' guanosinecap but not by the addition of a poly(A) tail (26). AlthoughTBSV has similar structural and genetic elements to BYDV-PAV,the 3'TE, which has also been identified in the genomes of boththe necroviruses and the dianthoviruses, is not present in theTBSV genome (26). The mechanism(s) by which the p33 and p92products of TBSV are expressed efficiently in vivo from a genomewhich lacks traditional translational enhancement elements istherefore unknown.

From previous studies, roles for p33 and p92 in TBSV genome replication have been inferred (22); however the evidence wasnot unequivocal. In the present study, we have further investigatedthe function of p33 and p92 and provide more definitive evidencethat both products are essential for viral RNA amplification.In addition, we have identified a 3' RNA segment within the TBSVgenome which has properties that are consistent with a potentialrole as a translational enhancer. Finally, our data provide novelinformation on important cis-acting sequences within viral RNAsas well as on functionally relevant regions of p33.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Viral and DI RNA constructs. Plasmid constructs T-100 and K2/M5, containing cDNAs corresponding to the full-length viral genomes of TBSV and cucumber necrosisvirus (CNV), respectively, have been described previously (6,16). HS-175 is a mutant of T-100 in which the amber stop codonfor the p33 ORF has been mutated to a tyrosine codon via a single-basesubstitution (22). Defective interfering (DI) RNA clones DI-82and DI-83, both of which encode p33, have been described previously,as have DI-73 and DI-72, which represent two small prototypicalTBSV DI RNAs (10, 28).

83 $Delta$ MfeI was constructed by digesting DI-83 with MfeI (at position 262 of the TBSV genomic sequence [6]) followed by fillingin of the 3'-recessed ends with T4 DNA polymerase and then self-ligation.The resulting construct, DI-83 $Delta$ MfeI, contained a 4-nucleotideinsertion at the MfeI site, causing a frameshift in the p33 ORF.For construction of DI-83M1, DI-83 was digested with BspEI (position993) followed by filling in of the 3'-recessed ends with T4 DNApolymerase and then self-ligation. The resulting construct, DI-83M1,contained a 4-nucleotide insertion at the BspEI site, causinga frameshift in the p33 ORF. To create DI-83M2, DI-83 was digestedwith BspEI and StuI (position 1059) and the 5' protruding endgenerated by BspEI was made blunt by filling in with T4 DNA polymerasefollowed by self-ligation of the gel-purified larger fragment.This created a construct, DI-83M2, that contained a 64-nucleotidedeletion of residues 997 to 1060, which resulted in a frameshift.To construct DI-83M3, DI-83 was digested with Tth111I (position928) and StuI and the 5' overhang of Tth111I was filled in withT4 DNA polymerase. The larger fragment was gel purified and thenself-ligated. The resulting construct, DI-83M3, contained a somewhatlarger than expected deletion of 177 nucleotides, correspondingto positions 899 to 1075 and resulting in a shift in the readingframe. DI-83CNV was constructed in the following manner. K2/M5was digested with StuI (position 1045) (16) and SphI (withinthe vector, 3' to the CNV cDNA insert), and the larger vector/5'-CNVsequence-containing fragment was gel purified and ligated to agel-purified StuI-SphI fragment (position 1059 to a more 3' positionwithin the vector) derived from digestion of DI-83. This generateda CNV/DI-83 hybrid molecule which contained the 5' end of theCNV genome (which encodes p33 of CNV) fused to the 3' portionof DI-83.

In vitro transcription. Viral transcripts were generated in vitro via transcription of SmaI-linearized template DNAs with the Ampliscribe T7 RNA polymerasetranscription kit (Epicentre Technologies). Following the transcriptionreaction, DNA templates were removed by treatment with DNase I(Epicentre Technologies) and unincorporated nucleotides were removedvia column chromatography with a Sephadex G-25 spin column (Pharmacia).Ammonium acetate was added to the flowthrough to a final concentrationof 2 M, and the transcripts were extracted twice with equal volumesof phenol-chloroform-isoamyl alcohol and then precipitated withethanol. Subsequently, the transcripts were quantified spectrophotometricallyand an aliquot was analyzed by agarose gel electrophoresis toverify integrity. Capped transcripts were prepared with the AmpliscribeT7 RNA polymerase transcription kit (Epicentre Technologies) byusing the recommended 10:1 ratio of cap analog [m⁷G(5')ppp(5')G; New England Biolabs] to GTP. Under these conditions,the manufacturer estimates an average capping efficiency of 50%.

Isolation and inoculation of protoplasts. Protoplasts were prepared from 6- to 8-day-old cucumber cotyledons (var. Straight 8) as described previously (8). Briefly,the lower epidermis of the cotyledons was peeled off with forcepsand the cotyledons were digested in 20 ml of an enzyme mix (0.25g of cellulase [Calbiochem], 0.025 g of pectinase [ICN], 0.025g of bovine serum albumin [ICN]) for 3 to 5 h with gentle shaking(40 rpm) in the dark. The protoplasts were then washed in 10%mannitol and purified by banding twice on a 20% sucrose cushion.Quantification was carried out by bright-field microscopy witha hemacytometer. Purified protoplasts (approximately 3 × 10⁵) were inoculated as described previously (8) with viral RNAtranscripts (1 µg for DI-72 or DI-73; 5 µg for the others) andwere incubated in a growth chamber under fluorescent lightingat 22°C for 24 h.

Analysis of viral RNAs. Total nucleic acid was harvested from protoplasts 24 h postinoculation by resuspension in 300 µl of a buffer containing 2×STE (28) and 1% sodium dodecyl sulfate. After two extractionswith phenol-chloroform-isoamyl alcohol, 100 µl of 8 M ammoniumacetate was added to the aqueous phase and the mixture was precipitatedwith ethanol. Aliquots (1/10) of the total nucleic acid preparationwere separated in nondenaturing 1.4% agarose gels. Viral RNAswere detected by electrophoretic transfer to nylon (Hybond-N;Amersham) followed by Northern blot analysis with a ³²P-end-labeled oligonucleotide (P9) probe complementary to the3'-terminal 23 nucleotides of the TBSV genome.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Viral RNA amplification via complementation of p33 and p92. It was suggested previously that the gene products of both ORF1 and ORF2 are required for replication of the TBSV genome (22).This conclusion was based on the observation that mutant genomeswhich allow for the expression of either p33 or p92 do not accumulatewhen tested individually. HS-175 is a mutant TBSV genome thatencodes only p92 due to the substitution of a tyrosine codon forthe amber stop codon of the p33 ORF. Previously, it was observedthat HS-175 does not accumulate when inoculated into protoplasts,and it was suggested that this result was likely a consequenceof a defect in replication resulting from the absence of p33 (22).There are, however, equally plausible alternative explanationsfor this observation. For example, the genome modification introducingthe tyrosine codon could cause (i) the production of a nonfunctionalp92, (ii) the destabilization of the genome, (iii) negative effectson translation, and/or (iv) the disruption of a promoter sequence.

In order to determine more definitively whether both p33 and p92 are required for genome amplification, we tested the abilityof mutant genomes, expressing either p33 or p92, to complementone another. Transcripts of the nonviable TBSV mutant HS-175 (Fig.1), encoding p92, were coinoculated with either of the independentlynonreplicable defective RNAs DI-82 and DI-83 (Fig. 1), both ofwhich encode p33. Structurally, these two defective RNAs differonly in their 3' regions, where a 167-nucleotide RNA segment,designated region 3.5, is present in DI-83 but is absent in DI-82.Protoplasts were coinoculated with various combinations of theseviral transcripts, total nucleic acids were isolated 24 h postinoculation,and viral RNAs were detected by Northern blotting (Fig. 2). Theinoculation with transcripts of wild-type (wt) TBSV genome (T-100)resulted in the accumulation of gRNA and its two sg mRNAs (Fig.2). Individual inoculations of HS-175, DI-83, or DI-82 resultedin no detectable viral RNA accumulation. Coinoculation of eitherDI-82 or DI-83 with T-100 resulted in significant accumulationof defective RNA progeny, indicating that both of these moleculescan be amplified efficiently in trans. When both DI-82 and DI-83were coinoculated with T-100, DI-82 clearly dominated. The HS-175/DI-83coinoculation, but not the HS-175/DI-82 coinoculation, led tosignificant accumulation of viral RNA (Fig. 2). In the HS-175/DI-83coinoculation, only DI-83 accumulated to readily detectable levels;however, very small amounts of HS-175 were detectable after longerexposures of the blots (data not shown). Interestingly, DI-82accumulation clearly dominated over that of DI-83 in the HS-175/DI-82/DI-83coinoculation, similar to that observed in the T-100/DI-82/DI-83coinoculation. It has been suggested previously that such differencesin competitiveness are related primarily to replication competence(28). The observation that viral RNA amplification occurredonly when the inocula contained both p33- and p92-encoding mutantsis consistent with the concept that complementation occurred andthat both products are necessary for the productive viral RNAamplification. Furthermore, these data indicate that expressionof functional p33 and p92 can be uncoupled. Sequence analysisof reverse transcription-PCR products of the readthrough region,which were amplified from progeny HS-175 isolated from severalindependent coinfections, showed that the tyrosine codon was maintainedin these molecules, thus indicating that reversion to wt had notoccurred at significant levels (data not shown).

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FIG. 2. Northern blot analysis of progeny viral RNAs isolated from cucumber protoplasts inoculated with various combinations of viral RNA transcripts. The RNA transcripts used in the inoculations are indicated at the top, and the positions of the genome (gRNA), sg mRNAs (sgRNA1 and sgRNA2), and defective RNAs (DI-82 and DI-83) are shown at the left. Total nucleic acids were isolated from approximately 3 × 10⁵ protoplasts after a 24-h incubation, separated in nondenaturing 1.4% agarose gels, transferred to a nylon membrane, and hybridized with a ³²P-labeled oligonucleotide probe complementary to the 3'-terminal 23 nucleotides of the TBSV genome.

To verify further that clone HS-175 was incapable of producing any p33, either by proteolytic cleavage of p92 or by prematuretermination of translation, and that functional p33 was indeedbeing provided by DI-83, a mutant of DI-83 was constructed inwhich p33 was inactivated. The mutant, DI-83 $Delta$ MfeI, contains aframeshift early in the p33 ORF, which would severely truncatethe product (Fig. 1). This mutant is predicted to encode onlythe N-terminal 33 amino acids (aa; plus an additional 18 non-p33C-terminal residues) of the normally 296-aa p33. When DI-83 $Delta$ MfeIwas coinoculated with HS-175, no viral RNA accumulation was detected(Fig. 3), even after longer exposures (data not shown). Coinoculationof HS-175/DI-83 demonstrated that the HS-175 transcripts usedin HS-175/DI-83 $Delta$ MfeI coinoculations were biologically active andcapable of complementation. Since 83 $Delta$ MfeI RNA accumulation wasobserved when 83 $Delta$ MfeI was coinoculated with T-100 (Fig. 3), itseems likely that the lack of amplification of DI-83 $Delta$ MfeI in coinfectionswith HS-175 is due to the absence of functional p33 rather thanto a defect in a cis promoter element. This finding further supportsthe concept that p33 is required for viral RNA amplification andthat in coinoculations with HS-175, functional p33 is being providedby DI-83.

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FIG. 3. Northern blot analysis of progeny viral RNAs isolated from cucumber protoplasts inoculated with various combinations of viral RNA transcripts. The RNA transcripts used in the inoculations are indicated at the top, and the positions of the genome (gRNA), sg mRNAs (sgRNA1 and sgRNA2), and defective RNAs (DI-83) are shown at the left. The position of DI-83 $Delta$ MfeI is the same as that indicated for DI-83. Total nucleic acids were isolated and analyzed as described in the legend to Fig. 2.

The activity induced by complementation can amplify DI-72 or DI-73. To investigate further the properties of the amplification activity in HS-175/DI-83 coinoculations, we tested whether it couldact on other amplifiable viral RNAs. DI-72 and DI-73 (Fig. 1)are two small DI viral RNAs which, when coinoculated with wt genomes,are amplified very efficiently (28). Assessment of the levelsto which DI-72 and DI-73 accumulate in coinoculations providesa very sensitive means of monitoring replicase activity. Variouscombinations of viral RNA transcripts were inoculated into protoplasts,and the levels of viral RNA accumulation were determined. EitherDI-72 or DI-73 accumulated very efficiently when coinoculatedwith T-100; however, both notably suppressed the accumulationof genomic and subgenomic RNAs (Fig. 4), as observed previously(28). These small DI RNAs also accumulated well when coinoculatedwith HS-175/DI-83 and showed a corresponding suppression of DI-83accumulation (Fig. 4). The efficient accumulation of DI-72 andDI-73 indicates that the amplification activity induced by complementationis not only able to act on replicons which encode p33 (i.e., DI-82and DI-83) but is also able to work efficiently in trans on otherviral RNA templates. No accumulation of either DI-72 or DI-73was observed when either was coinoculated with HS-175 or withHS-175/DI-82, further supporting the concept that HS-175, aloneor in combination with DI-82, is incapable of directing viralRNA amplification.

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FIG. 4. Northern blot analysis of progeny viral RNAs isolated from cucumber protoplasts inoculated with various combinations of viral RNA transcripts. The RNA transcripts used in the inoculations are indicated at the top, and the positions of the genome (gRNA), sg mRNAs (sgRNA1 and sgRNA2), and various defective RNAs are shown at the left. Total nucleic acids were isolated and analyzed as described in the legend to Fig. 2.

Coinoculation of HS-175 and capped DI-82 allow for viral RNA amplification. Our results indicated that DI-83, but not DI-82, was able to complement HS-175 for viral RNA amplification. DI-82 is identicalto DI-83 except that it lacks a 3' segment, region 3.5, whichis present in DI-83. The apparent defect in DI-82 must thereforebe related to the absence of this RNA segment. One possible rolefor region 3.5 in viral RNA amplification is to act as a translationalenhancer for p33 production. To investigate this possibility,we synthesized 5'-capped transcripts of DI-82 and tested whetherthis modification (predicted to increase the translation efficiencyof p33) would lead to productive viral RNA amplification. Whencapped DI-82 RNA transcripts (DI-82C) were coinoculated with HS-175,accumulation of DI-82C progeny was observed; however it was significantlylower than that observed for DI-83 in the HS-175/DI-83 coinoculation(Fig. 5). Efficient accumulation of DI-72 and DI-73 was also observedwhen they were coinoculated individually with HS-175/DI-82C (Fig.5). These results show that the inability of DI-82 to complementHS-175 for viral RNA amplification can be partially compensatedfor by the presence of a 5' cap structure. In addition, thesedata suggest that the p33 encoded in DI-82 is functional; therefore,the previously observed inability of uncapped DI-82 to complementHS-175 could not have been because it encoded a defective p33ORF.

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FIG. 5. Northern blot analysis of progeny viral RNAs isolated from cucumber protoplasts inoculated with various combinations of viral RNA transcripts. The RNA transcripts used in the inoculations are indicated at the top (with capped transcripts indicated by the suffix C), and the positions of the genome (gRNA), sg mRNAs (sgRNA1 and sgRNA2), and various defective RNAs are shown at the left. Total nucleic acids were isolated and analyzed as described in the legend to Fig. 2.

Functional analysis of mutant forms of p33. To determine the functional importance of the highly conserved C-terminal portion of p33 (6), several mutations were introducedinto DI-83, which modified the encoded p33 ORF (Fig. 6A). Themutant transcripts were then coinoculated with either T-100 orHS-175 to determine if they were replicable and/or if they couldcomplement to allow for viral RNA amplification, respectively.DI-83M1 has a 4-nucleotide insertion at position 997, which createsa frameshift, resulting in the replacement of the C-terminal 19aa of the p33 ORF with 40 residues from an alternate reading frame.The mutant DI-83M2 contains a deletion of 64 nucleotides, correspondingto positions 997 to 1060, which truncates the C terminus of thep33 ORF by 19 aa and adds 1 residue (Ala) from an alternate readingframe. Mutant DI-83M3 has a 177-nucleotide deletion (positions899 to 1075), which leads to removal of 52 aa from the C terminusof the p33 ORF and adds 3 residues (Leu-Gly-Leu) from anotherreading frame.

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FIG. 6. (A) Schematic representation of wt and mutant forms of DI-83. DI-83M1 has a 4-nucleotide insertion at position 997, which creates a frameshift, resulting in the replacement of the C-terminal 19 aa of p33 (open box) with 40 residues from an alternate reading frame (adjoining black box). DI-83M2 contains a deletion (indicated by a gap) of 64 nucleotides corresponding to positions 997 to 1060, which truncates the C terminus of p33 by 19 aa and adds 1 residue (Ala) from an alternate reading frame. DI-83M3 has a 177-nucleotide deletion (indicated by a gap; positions 899 to 1075), which leads to removal of 52 aa from the C terminus of p33 and adds 3 residues (Leu-Gly-Leu) from another reading frame. DI-83CNV has the 5'-terminal region of DI-83 replaced by the corresponding region from the CNV genome (darker shading) and encodes the CNV p33. (B) Northern blot analysis of mutant forms of DI-83. The RNA transcripts used in the inoculations are indicated at the top, and the positions of the genome (gRNA), sg mRNAs (sgRNA1 and sgRNA2), and defective RNAs (DI-83) are shown at the left. The positions of the mutant defective RNAs (M1, M2, and M3) are approximately the same as, or slightly lower than, that indicated for DI-83. (C) Northern blot analysis of DI-83CNV. The transcripts used in the inoculations are indicated at the top, and the positions of the genome (gRNA), sgmRNAs (sgRNA1 and sgRNA2), and defective RNAs (DI-83CNV) are shown at the left. For both panels B and C, total nucleic acids were isolated and analyzed as described in the legend to Fig. 2.

When transcripts corresponding to each of these three mutants were coinoculated individually with T-100, each accumulatedto detectable levels, providing evidence that all were replicable(Fig. 6B). In coinoculations with T-100, DI-83M1 consistentlyaccumulated to significantly lower levels than did either DI-82M2or DI-83M3, suggesting that the modification to DI-83M1 did notablyaffect its viability. In coinoculations with HS-175, no viralRNA accumulation was detected for any of the mutants (Fig. 6B).Since these mutants were trans-amplifiable with wt helper (albeitDI-83M1 at reduced levels), the results suggest that the defectin amplification is related to the predicted C-terminal modificationsin the encoded p33 ORF and that the C-terminal region of p33 isimportant for its functional activity.

To examine whether a high degree of compatibility is required between p33 and p92, a mutant of DI-83, DI-83CNV (Fig. 6A),was constructed in which the 5' portion of DI-83 was replacedby the corresponding region from the genome of CNV (a closelyrelated Tombusvirus). DI-83CNV thus encodes the CNV p33 homologin place of the TBSV p33 (Fig. 6A). The p33 of CNV is 89.2% identicalto the p33 of TBSV at the amino acid level (6). To determinewhether these differences would affect viral RNA amplification,coinoculations of HS-175 and DI-83CNV were analyzed. These coinoculationsresulted in the efficient accumulation of DI-83CNV progeny, indicatingthat the CNV p33 is compatible with the TBSV p92 (Fig. 6C).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, we have investigated the roles of p33 and p92 in the accumulation of TBSV RNAs. Our results suggest that bothof these proteins are essential for viral RNA accumulation, afinding consistent with their probable roles in viral RNA replication.The data also provide valuable information on important cis-actingsequences within viral RNAs as well as on functionally relevantregions of p33.

Both p33 and p92 are required for viral RNA amplification. By first uncoupling the expression of functional p33 and p92 to generate independently nonviable RNAs and then using complementationto restore viability, we have shown that both of these proteinsare likely required for amplification of the viral RNA. This conclusionis supported further by the observations that (i) the mutant DI-83 $Delta$ MfeI,containing an extensively truncated p33 ORF, could not complementHS-175 yet was able to replicate in trans with wt helper; (ii)no amplification was observed when HS-175 was coinoculated withthe normally efficiently replicating DI-72 or DI-73; and (iii)reverse transcription-PCR analysis of the readthrough portionof HS-175 indicated that no high levels of reversion of the tyrosinecodon had occurred in HS-175. These results indicate that thep92 expressed from HS-175 is functional and that p33 must be providedseparately. The data thus support the concept that both productsare required for viral RNA replication and that there is no strictprerequisite for their coupled expression.

The very low level of accumulation of HS-175 in HS-175/DI-83 coinoculations indicated that the nucleotide and/or codon substitutionintroduced into this RNA negatively impacts its viability. However,the efficient trans-amplification of DI-72 or DI-73 observed incoinoculations with HS-175 and DI-83 suggests that this low levelis not due to the inability of the amplification activity to actin trans on templates other than DI-83. It therefore seems likelythat this result may be due to altered properties of HS-175, whichrender it no longer able to accumulate efficiently (e.g., decreasedstability and/or disruption of a cis-acting replication element).In addition, it is plausible that assembly of the functional replicasecomplex occurs preferentially on the RNA template which encodesp33 but that once formed, the active complex is able to dissociatesubsequently and act on other templates (e.g., DI-72 and DI-73).Similar cis-preferential replication models, and the possibleadvantages thereof, have been discussed for turnip yellow mosaicvirus and TCV (27, 29).

The presence of polymerase-specific motifs in the readthrough portion of p92 has led to the suggestion that it representsa component of the viral RNA replicase (6). Amino acid sequenceanalysis of the p33 products of tombusviruses has indicated nosignificant relationship to any proteins of known function (18,25). Although the precise role of the TBSV p33 remains a mystery,it has been suggested that it may participate in genome replication(22). Results similar to those of this study were found whenp28, the TCV homolog of p33, was analyzed (29). The p28 productis also required, along with its readthrough product, p88, forviral RNA amplification. The prereadthrough proteins from theCarmovirus and Tombusvirus genera therefore appear to share certainkey properties and may have similar functions. In light of theseresults, it is conceivable that other members of the family Tombusviridaealso require both prereadthrough and readthrough products forproductive viral RNA amplification. It cannot, however, be entirelyprecluded that prereadthrough proteins may be functioning, alternativelyor additionally, via a mechanism independent of replication (e.g.,RNA stabilization).

Possible functional roles for region 3.5. Region 3.5 could represent an important component of a promoter. If this were true, the absence of region 3.5 in DI-82 andother highly replicable molecules, such as DI-72, indicates thatit would not be essential for trans-amplification of certain replicons.In fact, in various coinoculations, molecules lacking region 3.5are more competitive than their counterparts containing it (Fig.2) (28). It is possible that this region is important at anearly stage in the replication process, such as the initial assemblyof the replicase complex. Following assembly, region 3.5 may notbe strictly required for the initiation or elongation steps ofRNA synthesis on other RNA templates. Evidence contrary to thispossibility comes from studies on the closely related Tombusviruscymbidium ringspot virus (CyRSV) (11). Transgenic plants expressingonly the CyRSV p33 and p92 were able to support the amplificationof a CyRSV DI-72-like molecule (i.e., lacking its correspondingregion 3.5). This result suggests that in the transgenic system,some assembly of functional replicase is possible in the absenceof region 3.5; however, requirements under conditions of naturalinfections may differ.

It seems less likely that region 3.5 would represent a stability element, at least in the context of DI-82, since DI-82 isable to accumulate efficiently when coinoculated with T-100 andin other coinoculations. We have observed that capping DI-82 restoredits ability to complement HS-175. This provides support for theconcept that region 3.5 may act as a translational enhancer, similarto the 3'TE of BYDV-PAV (26). Interestingly, Scholthof and Jackson(19) found that modifications to the TBSV genome in a smallORF (encoding pX, a short polypeptide of unknown function), whichresides entirely within region 3.5, led to nonviability in certainhosts. It was also determined that disruption of the RNA sequence,rather than of the pX ORF, was responsible for these defects.In vitro translation studies showed that these mutations did notappreciably affect the expression of p33 (or p92), but a possiblerole in translational regulation in vivo was not ruled out. Unlikethe findings of the present study (Fig. 5), capping did not rescuethe viability of transcripts containing modifications to the pXORF (19). These differences in results may be related to variablesbetween the systems used in the two studies (e.g., differencesin hosts, viral RNAs, mutation types, and expression of p33 andp92). Studies are under way to delineate the sequences and/orstructures in region 3.5 which confer its complementation activityand to determine whether this element represents a translationalenhancer.

Functional and compatibility requirements of p33. Amino acid comparisons of p33 from three different tombusviruses (TBSV, CNV, and CyRSV) showed that the level of identitywas greatest in the C-terminal region (6). This high levelof conservation suggested a somewhat strict requirement for maintenanceof this region for functional activity. Three different mutationswere introduced into the C-terminal region of p33, and all moleculesharboring these modifications were unable to complement HS-175,yet all were amplified when coinoculated with T-100. These resultssuggest that the alterations to the p33 ORFs were responsiblefor the lack of viral RNA accumulation in the coinoculations.The smallest truncation in p33 that was not functional was onewhich removed 19 aa from the C terminus (DI-83M2), indicatingan important role for these residues. Replacement of the missing19 aa with 40 non-p33 residues (DI-83M1) did not restore the activity.These results suggest that the C-terminal ~6% of p33 is criticalfor its functional activity.

The expression strategy of p33 and p92 from the TBSV genome requires that the N-terminal region of p92 be identical to p33.If both these proteins are involved in replication, it is possiblethat there is some compatibility requirement between the two products.For the bromoviruses, it has been shown that the 1a and 2a viralreplication components interact directly (9) and that certaincompatibility requirements exist (2). If a direct interactionbetween p33 and p92 is required for TBSV, it would be mediatedby an association between either the two identical domains orp33 and the readthrough domain of p92. If the former were true,the overlapping nature of their ORFs would require that compatibilitybe maintained via a doubly coupled type of coevolution. If a compatibilityrequirement does exist between the TBSV p33 and p92, it is notexceptionally strict, since complementation was observed whenthe CNV p33 homolog was tested. This result also leaves open thepossibility that p33 functions independently of direct interactionwith p92.

	ACKNOWLEDGMENTS

We thank Laurie Baggio and members of our laboratory for reviewing the manuscript. We are also grateful to Herman Scholthoffor providing HS-175, D'Ann Rochon for providing K2/M5, and LoriWeisberg for constructing DI-83CNV.

This work was supported by grants to K.A.W. from the National Science and Engineering Research Council of Canada.

	ADDENDUM IN PROOF

Following submission of the final draft of this article, evidence suggesting a requirement for both the pre- and readthroughproducts of artichoke mottled crinkle Tombusvirus for genome amplificationwas presented (P. Molinari, C. Marusic, A. Lucioli, R. Tavazza,and M. Tavazza, J. Gen. Virol. 79:639-647, 1998).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biology, York University, 4700 Keele St., Toronto, Ontario, Canada M3J1P3. Phone: (416) 736-2100, ext. 40890 or 70352. Fax: (416) 736-5698.E-mail: kawhite{at}yorku.ca.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Dalmay, T., L. Rubino, J. Burgyan, A. Kollar, and M. Russo. 1993. Functional analysis of cymbidium ringspot virus genome. Virology 194:697-704[Medline].

2. Dinant, S., M. Janda, P. A. Kroner, and P. Ahlquist. 1993. Bromovirus RNA replication and transcription require compatibility between the polymerase- and helicase-like viral RNA synthesis proteins. J. Virol. 67:7181-7189[Abstract/Free Full Text].

3. Dolja, V. V., and J. C. Carrington. 1992. Evolution of positive-strand RNA viruses. Semin. Virol. 3:315-326.

4. Futterer, J., and T. Hohn. 1996. Translation in plants $---$ rules and exceptions. Plant Mol. Biol. 32:159-189[Medline].

5. Gorbalenya, A. E., E. V. Koonin, A. P. Donchenko, and V. M. Blinov. 1988. A conserved NTP-motif in putative helicases. Nature 333:22[Medline].

6. Hearne, P. Q., D. A. Knorr, B. I. Hillman, and T. J. Morris. 1990. The complete genome structure and synthesis of infectious RNA from clones of tomato bushy stunt virus. Virology 177:141-151[Medline].

7. Ishikawa, M., T. Meshi, T. Ohno, and Y. Okada. 1991. Specific cessation of minus-strand RNA accumulation at an early stage of tobacco mosaic virus infection. J. Virol. 65:861-868[Abstract/Free Full Text].

8. Jones, R. W., A. O. Jackson, and T. J. Morris. 1990. Defective-interfering RNAs and elevated temperatures inhibit replication of tomato bushy stunt virus in inoculated protoplasts. Virology 176:539-545[Medline].

9. Kao, C. C., and P. Ahlquist. 1992. Identification of the domains required for direct interaction of the helicase-like and polymerase-like RNA replication proteins of brome mosaic virus. J. Virol. 66:7293-7302[Abstract/Free Full Text].

10. Knorr, D. A., and T. J. Morris. 1991. De novo generation of defective interfering RNAs of tomato bushy stunt virus by high multiplicity passage. Virology 181:193-202[Medline].

11. Kollar, A., and J. Burgyan. 1994. Evidence that ORF 1 and 2 are the only virus-encoded replicase genes of cymbidium ringspot tombusvirus. Virology 201:169-172[Medline].

12. Koonin, E. V. 1991. The phylogeny of RNA-dependent RNA polymerases of positive-strand RNA viruses. J. Gen. Virol. 72:2197-2206[Abstract/Free Full Text].

13. Lupo, R., L. Rubino, and M. Russo. 1994. Immunodetection of the 33K/92K polymerase proteins in cymbidium ringspot virus-infected and transgenic plant tissue extracts. Arch. Virol. 138:135-142[Medline].

14. Maia, I. G., K. Seron, A. Haenni, and F. Bernardi. 1996. Gene expression from viral RNA genomes. Plant Mol. Biol. 32:367-391[Medline].

15. Miller, W. A., S. P. Dinesh-Kumar, and C. P. Paul. 1995. Luteovirus gene expression. Crit. Rev. Plant Sci. 14:179-221.

16. Rochon, D. M., and J. C. Johnston. 1991. Infectious transcripts from cloned cucumber necrosis virus cDNA: evidence for a bifunctional subgenomic promoter. Virology 181:656-665[Medline].

17. Rozanov, M. N., E. V. Koonin, and A. E. Gorbalenya. 1992. Conservation of the putative methyltransferase domain: a hallmark of the `Sindbis-like' supergroup of positive-strand RNA viruses. J. Gen. Virol. 73:2129-2134[Abstract/Free Full Text].

18. Rubino, L., J. Burgyan, and M. Russo. 1995. Molecular cloning and complete nucleotide sequence of carnation Italian ringspot tombusvirus genomic and defective interfering RNAs. Arch. Virol. 140:2027-2039[Medline].

19. Scholthof, H. B., and A. O. Jackson. 1997. The enigma of pX: a host-dependent cis-acting element with variable effects on tombusvirus RNA accumulation. Virology 237:56-65[Medline].

20. Scholthof, H. B., K. B. Scholthof, and A. O. Jackson. 1995. Identification of tomato bushy stunt virus host-specific symptom determinants by expression of individual genes from a potato virus X vector. Plant Cell 7:1157-1172[Abstract].

21. Scholthof, H. B., K. B. Scholthof, M. Kikkert, and A. O. Jackson. 1995. Tomato bushy stunt virus spread is regulated by two nested genes that function in cell-to-cell movement and host-dependent systemic invasion. Virology 213:425-438[Medline].

22. Scholthof, K.-B. G., H. B. Scholthof, and A. O. Jackson. 1995. The tomato bushy stunt virus replicase proteins are coordinately expressed and membrane associated. Virology 208:365-369[Medline].

23. Skuzeski, J. M., L. M. Nichols, and R. F. Gesteland. 1990. Analysis of leaky viral translation termination codons in vivo by transient expression of improved $beta$ -glucuronidase vectors. Plant Mol. Biol. 15:65-79[Medline].

24. Skuzeski, J. M., L. M. Nichols, R. F. Gesteland, and J. F. Atkins. 1991. The signal for a leaky UAG stop codon in several plant viruses includes the two downstream codons. J. Mol. Biol. 218:365-373[Medline].

25. Tavazza, M., A. Lucioli, A. Calogero, A. Pay, and R. Tavazza. 1994. Nucleotide sequence, genomic organization and synthesis of infectious transcripts from a full-length clone of artichoke mottled crinkle virus. J. Gen. Virol. 75:1515-1524[Abstract/Free Full Text].

26. Wang, S., K. S. Browning, and W. A. Miller. 1997. A viral sequence in the 3'-untranslated region mimics a 5' cap in facilitating translation of uncapped mRNA. EMBO J. 16:4107-4116[Medline].

27. Weiland, J. J., and T. W. Dreher. 1993. Cis-preferential replication of the turnip yellow mosaic virus RNA genome. Proc. Natl. Acad. Sci. USA 90:6095-6099[Abstract/Free Full Text].

28. White, K. A., and T. J. Morris. 1994. Nonhomologous RNA recombination in tombusviruses: generation and evolution of defective interfering RNAs by stepwise deletions. J. Virol. 68:14-24[Abstract/Free Full Text].

29. White, K. A., J. M. Skuzeski, W. Li, N. Wei, and T. J. Morris. 1995. Immunodetection, expression strategy and complementation of turnip crinkle virus p28 and p88 replication components. Virology 211:525-534[Medline].

30. Zaccomer, B., A. Haenni, and G. Macaya. 1995. The remarkable variety of plant RNA virus genomes. J. Gen. Virol. 76:231-247[Abstract/Free Full Text].

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1.	Dalmay, T., L. Rubino, J. Burgyan, A. Kollar, and M. Russo. 1993. Functional analysis of cymbidium ringspot virus genome. Virology 194:697-704[Medline].
2.	Dinant, S., M. Janda, P. A. Kroner, and P. Ahlquist. 1993. Bromovirus RNA replication and transcription require compatibility between the polymerase- and helicase-like viral RNA synthesis proteins. J. Virol. 67:7181-7189[Abstract/Free Full Text].
3.	Dolja, V. V., and J. C. Carrington. 1992. Evolution of positive-strand RNA viruses. Semin. Virol. 3:315-326.
4.	Futterer, J., and T. Hohn. 1996. Translation in plants $---$ rules and exceptions. Plant Mol. Biol. 32:159-189[Medline].
5.	Gorbalenya, A. E., E. V. Koonin, A. P. Donchenko, and V. M. Blinov. 1988. A conserved NTP-motif in putative helicases. Nature 333:22[Medline].
6.	Hearne, P. Q., D. A. Knorr, B. I. Hillman, and T. J. Morris. 1990. The complete genome structure and synthesis of infectious RNA from clones of tomato bushy stunt virus. Virology 177:141-151[Medline].
7.	Ishikawa, M., T. Meshi, T. Ohno, and Y. Okada. 1991. Specific cessation of minus-strand RNA accumulation at an early stage of tobacco mosaic virus infection. J. Virol. 65:861-868[Abstract/Free Full Text].
8.	Jones, R. W., A. O. Jackson, and T. J. Morris. 1990. Defective-interfering RNAs and elevated temperatures inhibit replication of tomato bushy stunt virus in inoculated protoplasts. Virology 176:539-545[Medline].
9.	Kao, C. C., and P. Ahlquist. 1992. Identification of the domains required for direct interaction of the helicase-like and polymerase-like RNA replication proteins of brome mosaic virus. J. Virol. 66:7293-7302[Abstract/Free Full Text].
10.	Knorr, D. A., and T. J. Morris. 1991. De novo generation of defective interfering RNAs of tomato bushy stunt virus by high multiplicity passage. Virology 181:193-202[Medline].
11.	Kollar, A., and J. Burgyan. 1994. Evidence that ORF 1 and 2 are the only virus-encoded replicase genes of cymbidium ringspot tombusvirus. Virology 201:169-172[Medline].
12.	Koonin, E. V. 1991. The phylogeny of RNA-dependent RNA polymerases of positive-strand RNA viruses. J. Gen. Virol. 72:2197-2206[Abstract/Free Full Text].
13.	Lupo, R., L. Rubino, and M. Russo. 1994. Immunodetection of the 33K/92K polymerase proteins in cymbidium ringspot virus-infected and transgenic plant tissue extracts. Arch. Virol. 138:135-142[Medline].
14.	Maia, I. G., K. Seron, A. Haenni, and F. Bernardi. 1996. Gene expression from viral RNA genomes. Plant Mol. Biol. 32:367-391[Medline].
15.	Miller, W. A., S. P. Dinesh-Kumar, and C. P. Paul. 1995. Luteovirus gene expression. Crit. Rev. Plant Sci. 14:179-221.
16.	Rochon, D. M., and J. C. Johnston. 1991. Infectious transcripts from cloned cucumber necrosis virus cDNA: evidence for a bifunctional subgenomic promoter. Virology 181:656-665[Medline].
17.	Rozanov, M. N., E. V. Koonin, and A. E. Gorbalenya. 1992. Conservation of the putative methyltransferase domain: a hallmark of the `Sindbis-like' supergroup of positive-strand RNA viruses. J. Gen. Virol. 73:2129-2134[Abstract/Free Full Text].
18.	Rubino, L., J. Burgyan, and M. Russo. 1995. Molecular cloning and complete nucleotide sequence of carnation Italian ringspot tombusvirus genomic and defective interfering RNAs. Arch. Virol. 140:2027-2039[Medline].
19.	Scholthof, H. B., and A. O. Jackson. 1997. The enigma of pX: a host-dependent cis-acting element with variable effects on tombusvirus RNA accumulation. Virology 237:56-65[Medline].
20.	Scholthof, H. B., K. B. Scholthof, and A. O. Jackson. 1995. Identification of tomato bushy stunt virus host-specific symptom determinants by expression of individual genes from a potato virus X vector. Plant Cell 7:1157-1172[Abstract].
21.	Scholthof, H. B., K. B. Scholthof, M. Kikkert, and A. O. Jackson. 1995. Tomato bushy stunt virus spread is regulated by two nested genes that function in cell-to-cell movement and host-dependent systemic invasion. Virology 213:425-438[Medline].
22.	Scholthof, K.-B. G., H. B. Scholthof, and A. O. Jackson. 1995. The tomato bushy stunt virus replicase proteins are coordinately expressed and membrane associated. Virology 208:365-369[Medline].
23.	Skuzeski, J. M., L. M. Nichols, and R. F. Gesteland. 1990. Analysis of leaky viral translation termination codons in vivo by transient expression of improved $beta$ -glucuronidase vectors. Plant Mol. Biol. 15:65-79[Medline].
24.	Skuzeski, J. M., L. M. Nichols, R. F. Gesteland, and J. F. Atkins. 1991. The signal for a leaky UAG stop codon in several plant viruses includes the two downstream codons. J. Mol. Biol. 218:365-373[Medline].
25.	Tavazza, M., A. Lucioli, A. Calogero, A. Pay, and R. Tavazza. 1994. Nucleotide sequence, genomic organization and synthesis of infectious transcripts from a full-length clone of artichoke mottled crinkle virus. J. Gen. Virol. 75:1515-1524[Abstract/Free Full Text].
26.	Wang, S., K. S. Browning, and W. A. Miller. 1997. A viral sequence in the 3'-untranslated region mimics a 5' cap in facilitating translation of uncapped mRNA. EMBO J. 16:4107-4116[Medline].
27.	Weiland, J. J., and T. W. Dreher. 1993. Cis-preferential replication of the turnip yellow mosaic virus RNA genome. Proc. Natl. Acad. Sci. USA 90:6095-6099[Abstract/Free Full Text].
28.	White, K. A., and T. J. Morris. 1994. Nonhomologous RNA recombination in tombusviruses: generation and evolution of defective interfering RNAs by stepwise deletions. J. Virol. 68:14-24[Abstract/Free Full Text].
29.	White, K. A., J. M. Skuzeski, W. Li, N. Wei, and T. J. Morris. 1995. Immunodetection, expression strategy and complementation of turnip crinkle virus p28 and p88 replication components. Virology 211:525-534[Medline].
30.	Zaccomer, B., A. Haenni, and G. Macaya. 1995. The remarkable variety of plant RNA virus genomes. J. Gen. Virol. 76:231-247[Abstract/Free Full Text].