Polymerase Slippage at Vesicular Stomatitis Virus Gene Junctions To Generate Poly(A) Is Regulated by the Upstream 3'-AUAC-5' Tetranucleotide: Implications for the Mechanism of Transcription Termination

doi:10.1128/JVI.75.15.6901-6913.2001

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Journal of Virology, August 2001, p. 6901-6913, Vol. 75, No. 15
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.15.6901-6913.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Polymerase Slippage at Vesicular Stomatitis Virus Gene Junctions To Generate Poly(A) Is Regulated by the Upstream 3'-AUAC-5' Tetranucleotide: Implications for the Mechanism of Transcription Termination

John N. Barr and Gail W. Wertz^*

Department of Microbiology, University of Alabama at Birmingham, Birmingham, Alabama 35294

Received 20 March 2001/Accepted 8 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Termination of mRNA synthesis in vesicular stomatitis virus (VSV), the prototypic rhabdovirus, is controlled by a 13-nucleotidegene end sequence which comprises the conserved tetranucleotide3'-AUAC-5', the U₇ tract and the intergenic dinucleotide. mRNAsterminated at this sequence possess 100- to 300-nucleotide-long3' poly(A) tails which are thought to result from polymerase slippage(reiterative transcription) by the VSV polymerase on the U₇ tract.Previously we determined that in addition to the AUAC tetranucleotide,the U₇ tract was an essential signal in the termination process.Shortening or interrupting the U₇ tract abolished termination.These altered U tracts also prevented the polymerase from performingreiterative transcription necessary for generation of the mRNApoly(A) tail and thus established seven residues as the minimumlength of U tract that allowed reiterative transcription to occur.In this study we investigated whether sequences other than theessential U₇ tract are involved in controlling polymerase slippage.We investigated whether the AUAC tetranucleotide affected theprocess of reiterative transcription by analyzing the nucleotidesequence of RNAs transcribed from altered subgenomic templatesand infectious VSV variants. The tetranucleotide was found toregulate reiterative transcription on the U₇ tract. The extentof polymerase slippage was governed not by specific tetranucleotidesequences but rather by nucleotide composition such that slippageoccurred when the tetranucleotide was composed of A or U residuesbut not when it was composed of G or C residues. This suggestedthat polymerase slippage was controlled, at least in part, bythe strength of base pairing between the template and nascentstrands. Further data presented here indicate that the tetranucleotidecontains both a signal that directs the VSV polymerase to slipon the downstream U₇ tract and also a signal that directs a slippingpolymerase to terminate mRNAsynthesis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Vesicular stomatitis virus (VSV) is one of the best-studied and best-characterized members of the order Mononegavirales, agroup which comprises RNA viruses having single-stranded genomesof negative-sense polarity. The 11,161-nucleotide VSV genome iscomposed of five genes flanked by leader and trailer sequencesarranged in the order 3' (leader)-N-P-M-G-L-(trailer) 5'. TheVSV RNA-dependent RNA polymerase (RdRp), comprised of the catalyticL protein component along with the P protein cofactor (10),binds to the nucleocapsid (N) protein encapsidated RNA templateat or near the genomic 3' terminus (9). The RdRp traversesthe VSV template in the 3'-to-5' direction, synthesizing a 47-nucleotideleader RNA, which is neither 5' capped nor 3' polyadenylated (6,7, 19), and five capped and polyadenylated mRNAs from eachof the VSV genes in a sequential fashion (1, 2, 38). Thefive VSV mRNAs are not transcribed with equal abundance; instead,due to a poorly understood process known as attenuation, genesnearer to the template 3' end are transcribed more frequentlythan those more 5' (18). There is much experimental evidenceto indicate that access to any downstream gene is possible onlywhen mRNA from the gene directly upstream has been transcribedand terminated by the same polymerase, and for this reason themodel which describes VSV mRNA synthesis is often referred toas stop-start transcription (1-4, 17).

Transcription by the VSV RdRp is controlled by sequences within the leader region, sequences at the leader-N gene junction,and sequences of the gene junctions (3, 4, 20, 24, 33,35, 41). The gene junctions comprise 23 highly conserved nucleotidesmade up of short sequences located at the end of an upstream geneand the beginning of a downstream gene. These sequences directthe VSV polymerase to polyadenylate and terminate the upstreammRNA, to initiate and cap the downstream mRNA, and are also responsible,at least in part, for the process of attenuation (3, 4,17, 27, 30, 31, 34-36).

The signal within the gene junction which specifies termination has been well studied and has been localized to 13 nucleotidescomprising a conserved tetranucleotide 3'-AUAC-5', a tract ofseven uridylates found at the end of each gene (the U₇ tract),and a dinucleotide 3'-GA-5' or 3'-CA-5' known as the intergenicsequence (3, 4, 17) which is not observed in either up-or downstream mRNA products. This wild-type termination signalis highly efficient, and so readthrough RNAs which arise whena termination signal is ignored are generated with a frequencyof only 1 to 3% (18). Gene junction sequences downstream ofthe termination signal have little effect on termination and areinvolved primarily in signaling initiation and correct processingof the nascent downstream mRNA 5' end (3, 35, 36).

Because of its sequence and its position at the end of each gene, the U₇ tract is thought to provide the template used togenerate the 100- to 300-nucleotide long 3' poly(A) tails thatare characteristic of VSV mRNAs (13-15, 23, 31). To accountfor the size of these tails relative to the short U₇ tract, theRdRp is believed to perform a cycle which involves realignmentof the template and polymerase such that the nascent strand movesbackward relative to the RdRp polymerization site, followed bycorrectly templated RNA synthesis. Repeated cycles of these twosteps allow synthesis of RNAs containing nontemplated nucleotides;this process is known as reiterative transcription or polymeraseslippage. Supporting the suggestion that reiterative transcriptionis responsible for the generation of VSV poly(A) tails, the VSVRdRp is known to perform this mode of transcription during otheraspects of RNA synthesis. Examples include synthesis of largepoly(A) tracts in readthrough RNAs synthesized in vitro and invivo (13, 14, 16, 32), generation of homopolymeric (U)sequences from a subgenomic template having an A₇ tract (3),and extensive copying of the sequence 3'-UUUUUAA-5' during G mRNAtranscription (5).

We previously investigated how changes within the conserved gene junction sequence affected transcription termination usingVSV subgenomic templates in a baby hamster kidney (BHK) cell-basedassay system (3). We found that termination of VSV mRNA synthesisdepended implicitly on the presence of the conserved U₇ tractand that shortening the tract to U₆ or interrupting it with anon-U nucleotide abolished termination, which led to exclusivesynthesis of a readthrough RNA (3). To determine why thesechanges abolished termination, we investigated whether the alteredU tract templates affected the ability of the VSV RdRp to performreiterative transcription; we found that slippage by the VSV RdRpwas abrogated by these changes and concluded that slippage toform the mRNA poly(A) tail was a crucial step in the terminationprocess. Furthermore, we demonstrated that slippage alone wasnot sufficient to cause termination, leading us to suggest thatthe VSV gene junction contained a signal which was required toallow a slipping polymerase to terminate synthesis of a correspondingmRNA.

In work described here, we have extended our previous studies and investigated whether sequences outside the U₇ tract canaffect polymerase slippage. Our results show that the upstream3'-AUAC-5' tetranucleotide of the gene junction exerts a majorinfluence on whether the VSV polymerase can slip on the downstreamU7 tract. Furthermore, our results suggest that the tetranucleotidesequence contains two or more signals that are required in combinationfor efficient termination: an element that allows initial polymeraseslippage on the U₇ tract, and an element that allows terminationof an RNA which is being reiterativelytranscribed.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmid constructions. Plasmid p8(+)NP, described previously (3, 4), directed bacteriophage T7 RNA polymerase to transcribe a positive-senseVSV subgenomic template containing the wild-type leader and trailerregions flanking two transcription units separated by a wild-typeN-P gene junction (Fig. 1A). This plasmid was constructed by positioningnucleotides 1 to 215, 1236 to 1686, and 10897 to 11161 of theVSV genome between a T7 RNA polymerase promoter and the cDNA encodingthe self-cleaving ribozyme from the antigenomic strand of hepatitisdelta virus. Following ribozyme cleavage, the T7 RNA polymerase-transcribedRNA had a 3' end which corresponded exactly with the 3' VSV genomicterminus but a 5' end that had two non-VSV nucleotides (GG). Asdescribed previously (3, 4), alterations were engineeredinto the gene junction sequence of p8(+)NP by exchanging a restrictionfragment spanning the gene junction sequence for a PCR-generatedfragment into which specific changes had been incorporated. Allalterations were confirmed by sequence analysis.

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FIG. 1. (A) Diagrammatic representation of the subgenomic template transcribed from plasmid p8(+)NP and the RNA products that it encodes. (A) The RNA template transcribed from p8(+)NP contains wild-type leader (le) and trailer (tr) regions flanking two transcriptional units, N/N and P/L, separated by the wild-type N-P gene junction. Plasmids encoding this and related subgenomic templates were transfected into vTF7-3-infected BHK cells, where they yielded positive-strand RNAs. These RNAs formed active templates by associating with supporting N, P, and L proteins encoded by transfected plasmids. Replication of the antigenomic RNA generated progeny negative-strand genomes which could act as templates for transcription or for generation of additional antigenomes by a further round of replication. All nucleotide alterations described in the text were made within the termination signal, shown 3'-5' in negative sense. (B) The subgenomic template transcribed from plasmid p8(+)NP transcribes positive-strand RNA transcripts; these are shown as actinomycin D-resistant, metabolically labeled RNAs harvested from BHK cells. The wild-type template (WT) transcribes a very low abundance of readthrough RNA; to indicate its position, RNAs transcribed from templates with tetranucleotide sequences 3'-AUAA-5' and 3'-AUAG-5' are shown alongside.

Plasmid pVSV-AUAC directed T7 RNA polymerase to generate a positive-sense antigenomic strand of an infectious recombinantVSV variant in which chloramphenicol acetyltransferase (CAT) andgreen fluorescent protein (GFP) genes were positioned immediatelyfollowing the leader region and separated by a wild-type genejunction sequence (see Fig. 7A). This plasmid was constructedby the stepwise insertion of two PCR-generated fragments containingthe CAT and GFP coding sequences, respectively, into the previouslydescribed plasmid pVSV(+)41 (40). Briefly, the CAT cDNA representedin plasmid pcDNA3CAT was amplified by PCR using oligonucleotideprimers CAT1 (5'-GTCACTCGAGTAAATGGAGAAGAAAATCACTGG-3') and CAT2(5'-ACGTACTAGTGCAAAAATTACGCCCCGCCCTGCCACTC-3'), and the resultingfragment was digested and inserted at the MseI and XhoI sitesof pVSV(+)41 to give plasmid pVSV(+)CAT. The GFP sequence representedin the previously described plasmid pVSV(+)1098 (40) was amplifiedby PCR using oligonucleotide primer GFP-1 (5'-TGACTCGAGCTACTAGTTATGAAAAAAACTAACAGATATCACCATGAGCAAGGGCGAGGAAC-3'),which annealed to the 3' end of the GFP gene, and oligonucleotideBstZ17I-n/c (5'-GTAAGAGATGTATACTCAATGTCATCAGGC-3'), which annealedto VSV N gene nucleotides 1017 to 1046. The amplified fragmentwas digested and inserted into the SpeI and BstZ17I sites of plasmidpVSV(+)CAT. Plasmids pVSV(+)GCGG and pVSV(+)AUAA, designed toexpress infectious recombinant VSV variants, were derived fromplasmid pVSV(+)AUAC by exchanging the SpeI- Bstz17I fragment describedabove for a fragment in which the wild-type gene junction 3'-AUAC-5'tetranucleotide sequence was replaced with 3'-AUAA-5', or 3'-GCGG-5'using an appropriately designed oligonucleotideprimer.

Transfections. Both single-round and budded-particle transfections were performed as described previously (26). Briefly, for generatingRNAs from single-round transfections, transcription plasmids encodingthe VSV N, P, and L proteins along with a specialized plasmidexpressing either a subgenomic or infectious virus template weretransfected into BHK cells expressing T7 RNA polymerase due toprior infection with vaccinia virus recombinant vTF7-3. For budded-particletransfections, support plasmids for N, P, M, G, and L proteinswere transfected into vTF7-3-infected BHK cells along with a subgenomictemplate-expressing plasmid. Budded particles released into thecell culture supernatant were used to infect a second vTF7-3-infectedBHK monolayer previously transfected with N, P, and L supportplasmids. This approach was taken to eliminate the generationof RNAs by T7 RNA polymerase and thus ensure that all RNAs whichcould act as templates for reverse transcriptase-mediated first-strandsynthesis were made by the VSV polymerase. Recombinant viruseswere recovered from corresponding cDNAs as described previously(42), and the nucleotide sequences of the resulting virus genomeswere confirmed by performing sequence analysis on purified viruspreparations.

Visualization of VSV specific RNAs. VSV-specific RNAs generated from subgenomic templates were labeled metabolically 16 h posttransfection by incubating transfectedand vTF7-3-infected BHK cells with [³H]uridine (33 µCi/ml) and actinomycin D (10 µl/ml) for 6 h asdescribed previously (26). RNAs generated from infectious recombinantVSV variants were labeled using the same approach except thatlabeling was performed at 2 h postinfection, for a total of 3h. Total cell RNA was harvested from monolayers using the RNeasypurification system (Qiagen Inc., Valencia, Calif.), and resultingRNAs were subjected to agarose-urea gel electrophoresis followedby fluorography and autoradiography (26).

Polymerase slippage assays. RNAs were analyzed for evidence of polymerase slippage using three approaches. The first assay used RNase H-directed cleavagein the presence of oligo(dT) to identify RNAs having additionalA residues that arise due to polymerase slippage on a templateU tract. This assay is based on the ability of RNase H to recognizeand cleave a short RNA-DNA hybrid. Briefly, ³H-labeled RNAs transcribed from subgenomic templates in first-roundtransfections were heated at 95°C for 1 min with 1 µg of oligo(dT)and then rapidly cooled on ice. Duplicate RNA samples withoutoligo(dT) were also prepared. After the addition of an equal volumeof 2× RNase H buffer (16) and 1 U of RNase H (Gibco-BRL), sampleswere incubated at 37°C for 20 min, after which they were purifiedand any resulting cleavage products were visualized by electrophoresisand fluorography as previously described (26).

A second approach detected evidence of polymerase slippage by determining the nucleotide sequence of individually cloned reversetranscriptase PCR (RT-PCR)-derived cDNAs. Briefly, first-strandcDNA synthesis was performed on magnetic bead-selected poly(A)⁺ readthrough RNAs (Miltenyi Biotech Inc., Auburn, Calif.), usinga modified Moloney murine leukemia virus reverse transcriptase(Superscript II; Gibco-BRL) and oligonucleotide pext-xba (5'-GCTCTAGACGAGAATAGGACTTGAGATACTCACG-3'),which annealed downstream of the VSV gene junction, at nucleotides1417 to 1450. Following purification, the cDNA population wasused as template for PCR amplification using oligonucleotidespext-xba and 9121-EcoR1 (5'-AACCGAATTCTGATATGATGCAGTATGCG-3'),which annealed upstream of the VSV gene junction, at VSV nucleotides1226 to 1254. PCR-amplified fragments were digested with restrictionenzymes XbaI and EcoRI and ligated into a similarly digested plasmidpGEM3. Single-nucleotide sequence analysis (using ddA chain terminator)was performed to detect whether slippage had occurred on the U₇tract. This same approach was used to sequence individual readthroughRNAs synthesized by infectious recombinant VSV variants exceptthat first-strand cDNA synthesis was primed using oligonucleotideeco-cloner (5'-ACGAGAATTCGGACCACGCCAGTGAACAGTTCC-5'), which annealedwithin the 3' end of the GFP gene. Subsequent PCR amplificationutilized oligonucleotides eco-cloner and xba-cloner (5'-TGATCTAGACGTGGCCAATATGACAACTTCTTCGCCCCCG-3'),which annealed within the 5' end of the CATgene.

The third slippage assay, termed the RT/Klenow assay, detected evidence of polymerase slippage by determining the spacingof two defined points on either side of the U₇ gene junction slippagesite (see Figure 4). Briefly, oligonucleotide pext-xba annealedto positive-sense readthrough RNAs downstream of the VSV genejunction to prime for [³⁵S]dATP-labeled first-strand cDNA synthesis using modified Moloneymurine leukemia virus reverse transcriptase (Superscript II; Gibco-BRL).After purification (PCR purification column; Qiagen), the labeledcDNA was primed for unlabeled second-strand cDNA synthesis usingoligonucleotide 9121 -eco and the Klenow fragment of DNA polymeraseI. After repeat purification, cDNAs were digested using restrictionenzymes EcoRV and StuI; the resulting DNA fragments were subjectedto polyacrylamide gel electrophoresis (PAGE) using a standardsequencing gel and visualized by autoradiography. RNAs derivedfrom infectious recombinant VSV variants were analyzed using thesame assay except that first-strand cDNA synthesis was primedusing oligonucleotide eco-cloner and second-strand synthesis wasprimed using oligonucleotide xba-cloner, both described above.The resulting cDNAs were digested with EcoRV and NcoI.

In each case, total cell RNAs were harvested as described above, treated with RQ1 DNase (Promega Corp., Madison, Wis.), andrepurified on an RNeasy column (Qiagen). All RNA samples wereconfirmed to be free of DNA by PCR (results notshown).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of subgenomic templates for investigation of polymerase slippage. As described above, we previously established that polymerase slippage on the essential U₇ tract of the VSV gene junctionwas a crucial part of the termination process. We also determinedthat templates in which the tetranucleotide (3'-AUAC-5') was changedto AUAA, AUAU, and AUAG were able to signal slippage but wereunable to signal termination, indicating that slippage alone wasnot sufficient to cause termination. To further investigate theprocess of transcription termination, we wanted to determine whetherchanges to the tetranucleotide sequence could affect slippageon the downstream U₇ tract, and if so, determine the role of thetetranucleotide in regulation of polymerase slippage. To achievethis, we generated a panel of subgenomic VSV templates derivedfrom the previously described plasmid p8(+)NP (3). This plasmid,shown diagrammatically in Fig. 1A, expressed a subgenomic VSVtemplate which contained two cistrons separated by the wild-typeVSV N-P gene junction. This template directed the transcriptionof two major mRNAs generated from the upstream (N/N) and downstream(P/L) cistrons, and also a minor readthrough RNA species synthesizedwhen the termination signals of the gene junction were ignored(Fig. 1B, AUAC). This readthrough RNA is the only transcriptionproduct generated from templates unable to terminate transcription,for example, those with the altered tetranucleotide sequencesAUAA and AUAG (3), shown in Fig. 1B. To investigate whetheralterations within the conserved tetranucleotide sequence of theVSV gene junction affected polymerase slippage, we constructedsubgenomic templates which contained the essential wild-type U₇slippage sequence (3) but contained altered tetranucleotidesequences located immediately upstream. We chose nucleotide alterationspreviously determined to lead to exclusive readthrough RNA synthesis;this was achieved by ensuring that the 5' C residue of the wild-type3'-AUAC-5' tetranucleotide was altered, thus abrogating terminationbut still allowing polymerase slippage (3).

Our decision to choose this design of template, and thus analyze the process of VSV polymerase slippage by analyzing readthroughRNAs, is based on the finding that VSV polymerase slippage isknown to occur during synthesis of readthrough RNAs in responseto template sequences (3). Therefore, by determining the extentto which reiterative transcription had occurred as the polymeraseencountered the essential U₇ slippage template in combinationwith a specific tetranucleotide sequence, we could assess theability of the corresponding templates to signal slippage. Thismethod of analysis is similar to that used to determine the sequencerequirements of paramyxovirus P gene editing, a related processthat is also governed by sequence signals within the template(12).

At this time, we did not address the question of how tetranucleotide alterations affected the degree of polymerase slippagethat occurred on a mRNA that was eventually terminated at thealtered gene junction. Such studies are complicated by the possibilitythat the 3' end of these terminated mRNAs will be modified byeither cellular processes or activities of recombinant vacciniavirus.

Rapid analysis of polymerase slippage using an RNase H digestion assay. To rapidly analyze a large number of subgenomic templates with altered tetranucleotide sequences for their ability to promotepolymerase slippage, we developed an assay based on a previousprocedure (22) which used RNase H in the presence of oligo(dT)to identify long stretches of poly(A) sequences within transcribedreadthrough RNAs. Although qualitative, this assay procedure wasattractive for two reasons. First, the assay analyzed all labeledRNAs in an RNA preparation, and thus the sample size was verylarge. Second, the assay did not depend on additional polymerasescommonly used to copy and amplify RNA sequences before theiranalysis.

By exposing [³H]uridine-labeled RNAs transcribed by T7 RNA polymerase in vTF7-3-infected BHK cells to RNase H in the presenceof oligo(dT), we determined that RNAs having A₉ or longer tractswere cleaved within this A tract to yield two faster-migratingRNAs (Fig. 2A). In contrast, RNAs with an A₆ or A₇ tract did notlead to the significant production of faster-mobility bands, indicatingthat these shorter A tracts were resistant to cleavage. The consequenceof this was that a readthrough RNA transcribed by the VSV polymerasefrom a subgenomic replicon that was a precise copy of the templatewould not be cleaved by RNase H since the RNA would have preciselyseven A residues at the position corresponding to the U₇ tract.Conversely, if the VSV polymerase had slipped during transcriptionof the readthrough RNA, the resulting species would contain additionalA residues and thus could be cleaved by RNase H, provided thatsufficient A residues were inserted. The replication productsgenerated from these templates are not visible in this systemand so do not contribute to the population of cleavedRNAs.

A group of 20 plasmids encoding subgenomic VSV templates with altered tetranucleotide sequences were constructed and individuallytransfected along with support plasmids expressing VSV N, P, andL proteins into BHK cells previously infected with recombinantvaccinia virus vTF7-3. After labeling of the VSV polymerase-generatedRNAs with [³H]uridine in the presence of actinomycin D, these RNAs were subjectedto the RNase H cleavage assay and agarose-urea gel analysis describedabove. Figure 2B shows the results of RNase H-oligo(dT) treatmenton RNA populations transcribed from three templates selected fromthis group having tetranucleotide sequences 3'-AGAA-5', 3'-AAAA-5'and 3'-CCCG-5'. The RNase H-oligo(dT) cleavage results of templatesAAAA and CCCG were selected because they represented the greatestand least cleavage, respectively, observed from the 20 templates.Template AGAA was selected because it represented an intermediatephenotype. These three templates directed exclusive transcriptionof the readthrough RNA, which is the only RNA species in lanesloaded with undigested RNA (Fig. 2B, lanes -). RNase H digestionof readthrough RNAs transcribed from template 3'-CCCG-5' did notresult in the production of the two characteristic cleaved RNAs;as described above, this indicated that slippage had not occurredduring readthrough RNA synthesis. In contrast, RNase H digestionproducts derived from readthrough RNAs transcribed from the template3'-AAAA-5' are clearly present, indicating that slippage occurredduring synthesis of these RNAs. RNase H cleavage of readthroughRNAs transcribed from the template 3'-AGAA-5' are faintly visible,indicating that a low level of slippage may have occurred duringtheir synthesis.

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FIG. 2. Analysis of VSV polymerase slippage by an RNase H-oligo(dT) digestion assay. (A) To determine what length of A tract was cleaved by RNase H in the presence of oligo(dT), positive-strand RNAs were transcribed in BHK cells by T7 RNA polymerase from four plasmids encoding subgenomic templates with gene junction U tracts of 6, 7, 9, and 14 nucleotides. These templates were transcribed to yield positive-stranded RNAs having corresponding A tracts of 6, 7, 9, and 14 nucleotides. Metabolically labeled RNAs were annealed to oligo(dT), digested with RNase H, and then visualized by agarose-urea gel electrophoresis and fluorography. Digestion of the labeled T7 RNA polymerase transcripts with an A₆ or A₇ tract was insignificant, whereas an expanded tract of nine A's was subjected to extensive digestion, as shown by the presence of two faster-migrating cleavage products. RNAs having A₁₄ tracts were digested to completion. (B) Metabolically labeled RNAs transcribed by the VSV polymerase from three subgenomic templates were subjected to the RNase H-oligo(dT) cleavage assay and visualized by agarose-urea gel electrophoresis and fluorography. The tetranucleotide sequences of gene junctions of these templates are shown above the corresponding lanes, written 3'-5'; + and $-$ denote presence and absence of oligo(dT). As described above, cleavage products following RNase H/oligo(dT) digestion were released only when the A tract contained more than seven residues. This assay demonstrated that VSV polymerase slippage was more prevalent on RNAs transcribed from the subgenomic template with the tetranucleotide sequence 3'-AAAA-5' than on templates with tetranucleotide sequence 3'-AGAA-5' or 3'-CCCG-5'. (C). RNAs transcribed from a total of 20 templates with altered tetranucleotide sequences were analyzed by the RNase H/oligo(dT) slippage assay, and the results were tabulated according to a qualitative assessment of whether digestion of the corresponding RNAs resembled the digestion pattern of RNAs transcribed from the three templates shown in panel 2B. AAAA-like corresponds to abundant digestion, CCCG-like corresponds to no detectable digestion, and AGAA-like corresponds to an intermediate level of digestion.

The primary results of RNase H-oligo(dT)-directed cleavage on readthrough RNAs transcribed from the other 17 templates ofthis group are not shown but are summarized in Fig. 2C, wherethese templates are categorized into three groups according towhich of the three templates shown in Fig. 2B best resembled theircorresponding pattern of RNAs following digestion. In this way,templates that transcribed RNAs that were subjected to a highdegree of cleavage were categorized as AAAA-like, templates transcribingRNAs that were not cleaved were grouped as CCCG-like, and templatesthat transcribed RNAs subjected to an intermediate degree of digestionwere grouped as AGAA-like. This classification indicated a trendin which readthrough RNAs transcribed from templates with A/U-richtetranucleotides were cleaved, whereas RNAs transcribed from templateswith G or C containing tetranucleotides were not cleaved. Templateswith tetranucleotides having a mixture of A/U and G/C nucleotidestranscribed RNAs exhibiting an intermediate degree of cleavage.These findings indicated that the tetranucleotide sequence wasable to affect the degree of cleavage of transcribed RNAs, whichin turn suggested that this sequence was able to affect the degreeof slippage that occurred on the downstream U₇tract.

Construction of the G/C and A/U groups of subgenomic templates. The results of the RNase H-oligo(dT) analysis described above suggested that the tetranucleotide sequence was able to affectthe occurrence of polymerase slippage on the U₇ tract. To furtherinvestigate the relationship between tetranucleotide sequenceand polymerase slippage, we generated a more extensive panel ofsubgenomic templates which had tetranucleotide sequences composedentirely of either A or U residues (the A/U group) or of G orC residues (the G/Cgroup).

Within the A/U group of templates, we restricted the 5'-most position of the A- and U-containing tetranucleotides to an Aresidue and in this way maintained the U tract as U₇ rather thanU₈ or longer. The three remaining positions of the A/U-containingtetranucleotide were varied to every possible permutation, generatingeight different subgenomic templates. For reasons discussed above,the 5' position of the 3'-AUAC-5' tetranucleotide in the G/C tetranucleotidetemplate group was restricted to a G residue to ensure that terminationdid not occur, and by using every possible permutation of G orC residues within the remaining three positions of this sequence,a further eight subgenomic templates were constructed. The precisesequences of the 16 altered tetranucleotides that were constructedare shown in Fig. 3. We assessed the extent of polymerase slippagedirected by these templates by using two different approachesas described below.

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FIG. 3. Subgenomic templates designed to exclusively transcribe readthrough RNAs. Subgenomic templates having tetranucleotide sequences composed of A and U residues (the A/U group) (A) and templates having tetranucleotide sequences composed of G and C residues (the G/C group) (B) were constructed and used to generate metabolically labeled and actinomycin D-resistant RNAs in BHK cells as described in Materials and Methods. RNAs were visualized by agarose-urea gel electrophoresis and fluorography. The altered tetranucleotide sequences (negative sense, 3'-5') of templates are shown above the lanes in which the corresponding RNAs products were electrophoresed. For reference, the wild-type termination sequence is shown, with the tetranucleotide sequence underlined. RNAs transcribed from subgenomic templates with tetranucleotide sequences AUAC (wild type) and AAAC, are shown alongside to indicate the mobility of terminated and readthrough RNAs. All tetranucleotide alterations within the A/U and G/C groups resulted in templates that directed exclusive synthesis of readthrough RNAs. In contrast to RNAs electrophoresed in Fig. 2B, the RNAs were not digested with RNase H.

Prior to assessing the extent of polymerase slippage, we determined that these subgenomic templates were unable to terminatemRNA synthesis at their altered gene junctions by visualizingthe actinomycin D-resistant, [³H]uridine-labeled RNAs they transcribed, using agarose-urea gelelectrophoresis followed by fluorography (Fig. 3). All of thetemplates within the G/C or A/U groups exclusively synthesizedthe previously characterized readthrough RNA, which indicatedthat the tetranucleotide alterations we had chosen had indeedprevented termination at the N/N geneend.

Further analysis of readthrough RNAs for evidence of VSV polymerase slippage. To further investigate the control of VSV polymerase slippage by the tetranucleotide sequence, we designed an assay (RT/Klenowassay [Fig. 4]) that precisely determined the length of the adenylatetract contained in readthrough RNAs. By analyzing the lengthsof poly(A) tracts within a bulk preparation of RNAs, this assayallowed us to assess the relative abundance that each A-tractlength represented out of the total population.

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FIG. 4. Schematic representation of the RT/Klenow slippage assay used to analyze RNAs for evidence of slippage by the VSV polymerase. 1, VSV genomes or subgenomic templates that included a potential slippage sequence (boxed) were used as templates for VSV polymerase-directed RNA synthesis. The slippage sequence comprised a U₇ tract preceded by a tetranucleotide sequence which was the site of all specific template alterations. 2, first-strand cDNA synthesis by reverse transcriptase in the presence of [³⁵S]dATP was primed using an oligonucleotide that annealed downstream of the slippage sequence. 3, labeled cDNAs acted as templates for unlabeled second-strand synthesis, using the Klenow fragment of E. coli DNA polymerase I to extend an oligonucleotide primer that annealed to a site corresponding to the upstream side of the slippage site. 4, resulting cDNAs were digested with restriction enzymes EcoRV and StuI. 5, digested cDNAs were denatured and subjected to PAGE and autoradiography to visualize the labeled cDNA fragments.

The RT/Klenow assay analyzed RNAs for the presence of additional nucleotides inserted at the U₇ slippage site by determiningthe spacing of two defined points within the readthrough RNA thatcorresponded to either sides of the gene junction in the template.This assay utilized a single polymerase (reverse transcriptase)to synthesize the labeled cDNA and thus reduced the potentialfor polymerase error to a minimum. Oligonucleotide primer pext-1annealed downstream of the gene junction and was extended usingreverse transcriptase in the presence of [³⁵S]dATP. After purification, the labeled first-strand cDNA wasprimed for unlabeled second-strand synthesis with oligonucleotide9121, using the Klenow fragment of DNA polymerase I. Purifiedduplex cDNAs were digested with restriction enzymes StuI and EcoRV,which recognized sites on either side of the potential slippagesequence, and cleaved cDNA fragments were analyzed by PAGE andautoradiography. The RNAs analyzed using this assay were generatedfrom subgenomic templates supplied as budded particles producedin a previous transfection rather than as T7 RNA polymerase transcriptssynthesized from plasmid cDNAs. This approach ensured that DNA-templatedRNAs produced by T7 RNA polymerase could not contribute to thepool of RNAs underanalysis.

We also carried out control experiments to determine whether slippage by T7 RNA polymerase had occurred during transcriptionof the subgenomic DNA templates. T7 RNA polymerase primary transcriptswere generated by transfecting template encoding cDNAs into vTF7-3-infectedBHK cells but without adding the VSV N, P, and L protein supportplasmids required for VSV-specific RNA synthesis. RNAs transcribedeither from budded-particle templates by the VSV polymerase orfrom plasmids by T7 RNA polymerase were concurrently analyzedusing the slippage assay. By this means, differences detectedbetween the two sets of resulting cDNA fragments could be attributedto the activity of the VSV polymerase, and in this way we wereable to rule out the possibility that slippage by T7 RNA polymerasehad contributed to the degree of slippage attributed to the VSVpolymerase.

Analysis of RNAs transcribed from the G/C group of templates. When subjected to the slippage assay described above, RNA transcripts generated from the eight subgenomic templates in theG/C group by both T7 and VSV RNA polymerases gave rise to a singlemajor species of labeled cDNA product (Fig. 5). The two sets ofcDNA bands exactly comigrated, indicating that the major RNAsproduced by both the T7 RNA and VSV polymerases were identicalin length (cDNA fragments generated from additional template CCCCare one nucleotide shorter due to the construction of this template).An additional cDNA band having a mobility indicating that it wasone nucleotide longer was also detected in all of the lanes, andthis band had an abundance between 5 and 10% of that of the majorspecies. This minor band most likely resulted from infrequentaddition of a single extra nucleotide at the slippage site byeither or both of the RNA polymerases or by reverse transcriptase.Because abundance of this minor band did not noticeably increasein the lanes specific for VSV polymerase-generated RNAs (Fig.5B) compared to the lanes specific for T7 RNA polymerase-generatedRNAs (Fig. 5A), we suggest that the addition is not likely causedby the VSV RNA polymerase. Whether T7 RNA polymerase or reversetranscriptase is responsible is unknown, although T7 RNA polymerasemust be a strong candidate, as instances of nontemplated nucleotideaddition by this polymerase have been previously reported in avariety of systems (21, 39).

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FIG. 5. RT/Klenow slippage assay analysis of RNAs transcribed from subgenomic templates with G/C tetranucleotides. (A) To control for slippage by either T7 RNA polymerase or reverse transcriptase, positive-stranded RNAs harvested from vTF7-3-infected BHK cells transfected with subgenomic template expressing cDNAs alone were subjected to the RT/Klenow slippage assay (Fig. 4). (B) To detect VSV polymerase slippage, RNAs transcribed from subgenomic templates supplied as budded particles were analyzed by the RT/Klenow slippage assay. The tetranucleotide sequences of altered subgenomic templates are shown beneath the corresponding lanes. For reference and as a control, templates unable to signal polymerase slippage due to their shortened U₅ and U₆ tracts were also included in the assay. The additional template CCCC produced RNAs one nucleotide shorter than others due to a deletion during construction of the corresponding cDNA.

As VSV polymerase slippage was not detected during transcription of these templates, we can conclude that the U₇ tract isnot sufficient to allow slippage on its own. This finding indicatesthat sequences outside the U₇ tract are involved in the regulationof polymerase slippage. Furthermore, when RNAs transcribed bythe VSV polymerase were analyzed using the slippage assay, thepattern of labeled bands did not noticeably vary between any ofthe eight templates, indicating that all of the correspondingtetranucleotide sequences were able to suppress VSV polymeraseslippage on the U₇ tract. Prevention of polymerase slippage wasthus a feature common to each of these altered tetranucleotidesequences, and we suggest this feature is the overall G/C contentof thissequence.

Analysis of RNAs transcribed from the A/U group of templates. Using the slippage assay described above, analysis of T7 RNA polymerase transcripts generated from the A/U group of templatesgave rise to a single major species of labeled product (Fig. 6A)similar to that seen with the G/C group of templates. Similarto the G/C group of RNAs described above, a minor cDNA band onenucleotide longer with an abundance of approximately 10% of thatof the major species was also present. As described above, thisspecies may have resulted from a low level of slippage by T7 RNApolymerase. If T7 RNA polymerase is the cause of this faint band,then slippage must be restricted to allow only a single nucleotideaddition and also must be a rare event.

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FIG. 6. RT/Klenow slippage assay analysis of RNAs transcribed from subgenomic templates with A/U tetranucleotides. To detect VSV polymerase slippage, RNAs were analyzed by the RT/Klenow slippage assay (Fig. 4) and also by determining the nucleotide sequence of RT-PCR-generated cDNA products. (A) To control for slippage by either T7 RNA polymerase or reverse transcriptase, RNAs harvested from vTF7-3-infected cells BHK cells transfected with only subgenomic template expressing cDNAs were subjected to the RT/Klenow slippage assay. (B). To detect slippage by the VSV polymerase, RNAs transcribed from templates supplied as budded particles were subjected to the RT/Klenow slippage assay. In both panels, the tetranucleotide sequences of the templates are shown beneath the corresponding lanes. RNAs transcribed from template AUAA were of faster mobility than those transcribed from other templates due to a four-nucleotide deletion in the cDNA. For reference and as a control, templates unable to signal polymerase slippage (U₅ and U₆) were included in the assay. To determine the number of A residues present in the A tracts of individual RNAs, RNAs synthesized by both VSV and T7 RNA polymerases from the template with the tetranucleotide 3'-AUAA-5' were used to generate RT-PCR fragments, which were cloned into pGEM3 and subjected to nucleotide sequence analysis. A total of 46 cDNAs generated by RT-PCR from T7 RNA polymerase transcripts (C) and 46 cDNAs generated by RT-PCR from VSV polymerase transcripts (D) were sequenced, and the results are shown in the form of a bar chart.

In marked contrast to the results of the G/C group, slippage analysis of the VSV polymerase transcribed RNAs from the A/Ugroup of templates gave rise to a series of labeled cDNA bandsthat gave the appearance of a ladder, extending upward in thegel (Fig. 6B). The mobility of these bands indicated that theycontained additional nucleotides, suggesting that the A/U-richtetranucleotide templates had allowed slippage to occur on theU₇ tract during synthesis of the correspondingRNAs.

The activities of the VSV polymerase on all eight of the A/U group of templates under assay appeared similar, despite thesetemplates having different tetranucleotide sequences. This findingindicated that promotion of VSV polymerase slippage was controlledby a feature common to all of the eight different templates, andwe suggest that this was the A/U content of thetetranucleotide.

Sequence analysis of cDNAs synthesized from T7 and VSV RNA polymerase-generated RNAs. Using the RT/Klenow assay described above, we analyzed large populations of RNA transcribed from altered subgenomic templatesin order to investigate how the tetranucleotide sequence was ableto control VSV polymerase slippage. While this assay allowed usto assess the relative extent to which polymerase slippage hadoccurred during transcription of a population of RNAs, it didnot allow us to precisely determine the exact number of nucleotidesadded during individual slippage events. To determine the extentto which polymerase slippage had occurred in individual instances,we determined the nucleotide sequences of 46 cDNA clones generatedby RT-PCR from populations of VSV-specificRNAs.

RT-PCR was performed on RNAs transcribed by the VSV polymerase in budded-particle transfections, and the sequences of individuallycloned cDNAs were determined. Because the RNA population transcribedfrom all members of the A/U group gave very similar patterns oflabeled cDNAs in the slippage assay, we performed sequence analysison only one template of this group, the one having the tetranucleotidesequence AUAA. As a control for polymerase slippage by T7 RNApolymerase, RNA transcripts of this template generated by thispolymerase were analyzed by the same procedure. We did not individuallyanalyze RNAs transcribed from members of the G/C group becausethese RNAs previously showed no signs of slippage in the RT/Klenowslippageassay.

The data in Fig. 6C show that T7 RNA polymerase synthesized a great majority (86%) of correctly sized RNAs with a tract ofseven U residues, with the remaining 14% having U tracts of eightnucleotides. The slightly higher proportion of U₈ to U₇ templatesthan previously estimated by the RT/Klenow slippage assay on thistemplate (Fig. 6A) may be due to either the relatively small numberof cDNA clones that were sequenced (46 clones) or errors introducedduring PCR amplification. In contrast, the RNAs generated by VSVpolymerase displayed greater heterogeneity of A-tract size, withonly 20% having the exact templated A-tract length of 7 (Fig.6D). The remaining 80% of the RNAs all had additional A residuespresent in their A tracts, with the longest A-tract length being40. The relative abundance of the RNAs that showed evidence ofpolymerase slippage by direct sequencing correlated with the resultsgenerated by the RT/Klenow slippage assay (Fig. 6A). Nucleotidesequence analysis of these cDNAs indicated that all additionalnucleotides detected in the readthrough RNAs were Aresidues.

Construction of recombinant VSV variants possessing an additional gene junction. In the previous sections we investigated how alterations of the tetranucleotide sequence affected the ability of the VSV polymeraseto slip on the adjacent U₇ tract. The assays were performed usingRNAs generated in the well-established subgenomic template systembecause it offered a combination of ease of template manipulationand biological authenticity (3, 4). However, to furtherstrengthen our findings, we also chose to analyze the occurrenceof VSV polymerase slippage during RNA synthesis by infectiousrecombinant VSV variants. This approach would allow us to investigatepolymerase slippage in a system that did not rely on coinfectionwith a vaccinia virus recombinant or the transient expressionof supporting proteins. In particular, the ability of vacciniavirus-encoded enzymatic activities to modify both 3' and 5' endsof RNAs were of potential concern, as the consequences of suchmodifications on VSV polymerase activity areunknown.

We constructed plasmids designed to generate recombinant VSV variants having two extra nonviral genes (CAT and GFP) separatedby a gene junction into which tetranucleotide alterations couldbe engineered without affecting the relative expression of thefive VSV genes further downstream (Fig. 7A). We selected one tetranucleotidesequence from each of the G/C and A/U groups of subgenomic templatesdescribed above, namely, GCGG and AUAA, and inserted these sequencesindependently at the CAT-GFP gene junction of the relevant cDNAsto create pVSV-GCGG and pVSV-AUAA, respectively. In addition,we constructed a cDNA designed to generate an infectious VSV variantin which the two additional genes were separated by the wild-typeVSV N-P gene junction sequence (pVSV-AUAC). Infectious viruseswere recovered from these cDNAs and used to infect BHK cells.The VSV-specific RNAs were labeled and visualized as previouslydescribed (42). The RNAs synthesized by the three recombinantVSV variants as well as from the wild-type VSV are shown in Fig.7B. VSV-AUAC-directed the transcription of two additional RNAproducts compared to the wild type, which corresponded to theindividual mRNAs transcribed from the CAT and GFP genes. In addition,a minor RNA of much slower mobility which represented the bicistronicCAT-GFP readthrough RNA was also detected on longer exposure ofthe gel. Compared to wild-type VSV, the VSV variants VSV-GCGGand VSV-AUAA expressed just one extra RNA of slower mobility whichrepresented the bicistronic CAT-GFP readthrough RNA.

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FIG. 7. Diagrammatic representation of recombinant VSV variants containing two additional transcriptional units, and visualization of the RNAs that these viruses encode. (A) CAT and GFP sequences were inserted into plasmid pVSV(+) to generate the recombinant virus VSV-AUAC, which contained two additional transcriptional units separated by a wild-type gene junction. Altered tetranucleotides 3'-AUAA-5' and 3'-GCGG-5' were engineered into the CAT-GFP gene junction of this cDNA (underlined) to generate the VSV recombinants VSV-AUAA and VSV-GCGG. (B) Metabolically labeled, actinomycin D-resistant RNAs transcribed from recombinant VSV variants in infected BHK cells were visualized by agarose-urea gel electrophoresis followed by fluorography. The VSV N, P, M, G, and L mRNAs are marked, along with the CAT, GFP, and bicistronic CAT-GFP readthrough RNAs synthesized from the additional transcriptional units. For reference, the RNAs transcribed by wild-type VSV (WT) are shown alongside.

Analysis of RNAs generated by the VSV variants. Readthrough RNAs generated by these three VSV variants in infected BHK cells were harvested and analyzed for evidence of polymeraseslippage. VSV-GCGG and VSV-AUAA synthesized abundant readthroughRNAs (Fig. 7B), and so RNAs expressed from these viruses wereanalyzed by the RT/Klenow slippage assay described above. Figure8A shows the labeled cDNA products of the slippage assay. ReadthroughRNAs transcribed from VSV-GCGG showed no evidence of polymeraseslippage, whereas RNAs transcribed from VSV-AUAA showed abundantevidence of slippage. These results were indistinguishable fromthose obtained using the plasmid-supported subgenomic templatesystem and thus confirmed our finding that G/C tetranucleotidesequences acted to prevent polymerase slippage, whereas A/U tetranucleotidesacted to promote slippage.

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FIG. 8. Analysis of RNAs transcribed by the VSV polymerase from recombinant viruses VSV-AUAC, VSV-GCGG, and VSV-AUAA which have altered tetranucleotide sequences within the CAT-GFP gene junction. (A) RNAs transcribed in infected BHK cells from viruses VSV-AUAA and VSV-GCGG were analyzed by the RT/Klenow slippage assay, and the radiolabeled cDNAs were visualized by PAGE analysis and autoradiography. The lanes are marked with the tetranucleotide sequence of the corresponding viruses. (B) Readthrough RNAs transcribed from recombinant virus VSV-AUAC were analyzed not by the slippage assay but by determining the nucleotide sequence of individual RT-PCR generated cDNAs due to the low abundance of the readthrough RNA species. A total of 51 RT-PCR-generated cDNA clones were sequenced, and the results are shown in a bar chart with the numbers on the horizontal axis corresponding to numbers of A residues detected in the A tract. The rounded percentage abundances of each A-tract length are as follows: A₇, 52%; A₈, 10%; A₁₀, A₁₁, and A₁₂, 4%; A₁₄ 6%; A₁₅, A₁₆, A₁₇, A₁₉, A₂₀, A₂₁, and A₂₂, 2%; and A₂₆₊, 8%.

VSV-AUAC generated a very low quantity of readthrough RNAs (Fig. 7B), and so these RNAs could not be analyzed by the RT/Klenowslippage assay. Instead, readthrough RNAs were analyzed by nucleotidesequencing of corresponding RT-PCR products. Briefly, polyadenylatedRNAs were selected by a magnetic bead poly(A) enrichment procedure,which was necessary to remove the positive-sense antigenome whichcould also act as template for the initial reverse transcriptionreaction. The poly(A)⁺ RNAs were used as the template for RT-PCR amplification, andthe resulting PCR products were inserted into pGEM3 and individuallysequenced. Of 51 cDNAs analyzed, 25 (49%) were found to have anunaltered A, sequence at the gene junction, indicating faithfulcopying of the gene junction U₇ tract, and a further 7 cDNAs (14%)showed the presence of a single additional A residue (Fig. 8B).The remaining 19 cDNAs contained A tracts that predominantly rangedbetween 10 and 22 nucleotides in length (3 of the 19 cDNAs hadA tracts of 31, 40, and 63 nucleotides), indicating that the tetranucleotideAUAC was able to signal polymerase slippage on the U₇ tract. However,by comparing Fig. 8B with Fig. 6D, we noted that the extent andfrequency of slippage on the AUAC template is less than that determinedfor the template with the AUAA tetranucleotide; a possible explanationof this finding is discussedbelow.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The weight of evidence suggests that the long poly(A) tails at the 3' ends of VSV mRNAs are synthesized by the VSV polymeraseperforming reiterative transcription, or polymerase slippage,on the relatively short U₇ tract located at each of the VSV genejunctions. Since mRNAs lacking poly(A) tails are not observedin wild-type VSV infections, polyadenylation and consequentlypolymerase slippage are both likely to be crucial steps in theprocess of VSV mRNA termination. In this study, we investigatedwhether sequences other than the U₇ tract affected the processof polymerase slippage by analyzing the nucleotide sequence ofRNAs transcribed from altered subgenomic templates and infectiousVSVvariants.

Our findings showed that the U₇ sequence alone was not sufficient to signal polymerase slippage and that the composition ofthe upstream tetranucleotide sequence (underlined) of the conservedVSV termination signal (3'-AUACUUUUUUUGA-5') was a major determinantof the degree of slippage that occurred on the downstream U₇ tract.Analysis of readthrough RNAs generated from templates having tetranucleotidescomposed entirely of various combinations of A and U residuesshowed extensive and frequent polymerase slippage. The extentto which slippage occurred was approximately the same for allof the eight A/U-containing templates tested, and we interpretthis to indicate that the ability of a template to promote polymeraseslippage on the U₇ tract was controlled by the upstream tetranucleotidein a way that did not depend on a precise sequence signal. Similarly,when we analyzed the readthrough RNAs transcribed from the groupof templates with tetranucleotide sequences composed entirelyof various combinations of G and C residues, we found that polymeraseslippage on the U₇ tract was prevented in all cases despite thevariety of tetranucleotide sequences. Therefore, for templateswithin these two groups, promotion or abrogation of polymeraseslippage did not depend on precise sequences within the tetranucleotide,which consequently indicated that the signal controlling slippagewas a common property of all members of the two individual groups.We suggest that this common element is overall G and C contentin the case of slippage abrogation and is overall A and U contentin the case of slippagepromotion.

How might these various tetranucleotide sequences alter the activity of the VSV polymerase and dictate whether or not it canslip on the U₇ tract? There are several possible mechanisms throughwhich this effect may be mediated. These include interaction ofthe template strand tetranucleotide with the complementary regionof the nascent strand or interaction of either of these sequenceswith the VSV polymerase, with an unidentified component of thehost cell, or with a trans-acting nucleic acidmolecule.

Our observation that A/U tetranucleotide sequences acted to promote slippage whereas G/C tetranucleotides prevented it makesit tempting to propose that polymerase slippage is controlled,at least in part, by the strength of an interaction between twonucleic acid molecules that are base paired. Because of theirproximity to the catalytic site of the VSV polymerase and theirability to form a perfectly base-paired hybrid, we suggest thatthe most likely candidates for these interacting molecules arethe genomic template and the nascent RNA strands. This interpretationcan accommodate our observation that tetranucleotide sequencessignaled the promotion or abrogation of slippage in a way thatwas independent of the exact tetranucleotide sequence, so longas the A/U or G/C nucleotide composition of this sequence wasmaintained. Clearly any alteration of the tetranucleotide wouldcause the corresponding alteration of the nascent strand, thusallowing maintenance of the base-pairing ability of template andnascent strands. If this hybrid strength is in fact the signal,then several tetranucleotide sequences would likely provide comparablesignals, which is in accordance with ourfindings.

As we stated above, alternative mechanisms by which tetranucleotide alterations could modulate polymerase slippage includeinteraction with components such as the VSV polymerase, a hostcell factor, or an additional nucleic acid molecule. However,in contrast to the template and nascent strands, components suchas these will obviously not change in accordance to an alterationin tetranucleotide sequence. Therefore, to permit the type ofsequence-independent signaling observed in this study, these componentswould need to be capable of recognizing, and responding consistentlyto, a broad range of RNA sequences. We consider this lesslikely.

If an interaction between the template and nascent strands is important in signaling polymerase slippage, do these findingstell us anything about the nature of such a hybrid? The precisenumber of nucleotides for which the template and nascent RNA strandsof VSV are hybridized during polymerization is not known. However,during the slippage reaction, it seems unlikely that the hybridcould extend for more than the seven residues of the U tract becauseas soon as even one round of polymerase slippage had occurred,unfavorable base pairing combinations would be required to formbetween newly inserted (and nontemplated) A residues and non-U(and thus noncomplementary) residues within the template strandtetranucleotide. Why then do changes within the tetranucleotidehave such a dramatic effect on polymerase slippage that suggestinvolvement in a hybrid? A possible answer is that the tetranucleotidemay exert its effect only immediately before an initial slippageevent takes place. At such a time, the nascent strand and thetemplate will be perfectly complementary, and perhaps a weak hybridextending across both the U₇ tract and an A/U-rich tetranucleotidemay provide sufficient instability to allow the initiation ofslippage. Once initial slippage has occurred, the length of thehybrid will be reduced to just the U₇ tract and its complement,and so potentially unfavorable base pairings are not requiredto form. In contrast, a G/C-containing tetranucleotide precedingthe U7 tract may prevent initial interstrand movement and thusprevent a slippageevent.

This explanation would imply that the number of nucleotides involved in the hybrid varies during the termination process.While there is currently no evidence to suggest that the VSV polymerasebehaves in this way, the RNA polymerase of Escherichia coli hasbeen shown to move backward in response to weak base-pairing potentialbetween the template and nascent strands, even when these nucleotidesextend upstream of an 8- or nine-nucleotide-long hybrid (25).It is conceivable that if such a mechanism existed in VSV, thenthe weak base pairing potential of an A/U-rich tetranucleotidemay allow realignment of the template and polymerase within theU₇ tract, and when followed by correctly templated RNA synthesis,cycles of this process could generate the expanded poly(A) tractsthat we haveobserved.

We previously analyzed how changes at the gene junction affected termination ability and established that while all changeswithin the tetranucleotide decreased termination ability comparedto that of the wild-type sequence, certain changes were more deleteriousthan others (3). We were unable to establish a pattern relatingtetranucleotide alteration to corresponding termination abilityand thus could not precisely predict how a defined alterationwould affect termination, and understanding this relationshiphas been one of our goals. In particular, we have been intriguedto understand why the single nucleotide alteration of the wild-typegene junction tetranucleotide 3'-AUAC-5' to one with the sequence3'-AUAA-5' decreased termination from 99% to 0%. Also, given theimportance of polymerase slippage in the termination process,we were curious to understand why tetranucleotide alterationsthat, according to the results of this study would not be expectedto alter slippage ability, had a major affect on termination.As an example, changing the tetranucleotide 3'-AUAC-5' to UUAC,AAAC, or AUUC leads to a 33% reduction in termination abilitycompared to that of wild type (3).

In an attempt to tie our observations together, we suggest that the tetranucleotide comprises at least two signals that arerequired for termination to occur and that these signals overlap.The first signal is high overall A/U content, which promotes interstrandslippage in the vicinity of the U₇ tract, and the second is asignal that allows polymerase molecules engaged in reiterativetranscription to terminate synthesis of the corresponding mRNA.We have termed this the commitment signal. This commitment signallikely includes the 5' C residue of the 3'-AUAC-5' tetranucleotide,since alteration of this position to any other residue resultsin the total loss of termination ability (3). However, we suggestthat the commitment signal also depends on the identity of theother three positions of the tetranucleotide, and this allowsus to explain why seemingly preserving potential slippage abilityof a tetranucleotide, as described above, can lead to a loss intermination ability. In these cases, the alterations have maintainedslippage potential, but as the two signals overlap, they haveperturbed the commitment signal. As any change of the tetranucleotidecan alter either or both of these two signals, precisely definingthe commitment signal in isolation is problematical. However,we know that the most efficient tetranucleotide sequence for terminationof mRNA synthesis is the wild-type sequence 3'-AUAC-5' (99% terminationability) (3, 4), and we suggest that this is because thissequence provides the most effective balance of the slippage andcommitment elements. The lessened ability of the AUAC tetranucleotideto promote polymerase slippage compared to AUAA (compare Fig.6D and 8B) is perhaps necessary to ensure the presence of theessential C residue that is obligately required for transcriptiontermination (3).

By what mechanism does the C residue of the tetranucleotide provide the essential termination signal? In the same way as describedabove for signaling slippage, the C residue may be involved ina crucial interaction within the template: nascent strand hybrid.Alternatively, the C residue of the template (or G residue ofthe nascent strand) may interact with either the VSV polymerase,a host cell component, or an unidentified nucleic acid molecule.However, in contrast to the signal that regulated polymerase slippage,which can be provided by several tetranucleotide sequences, thesignaling ability of the essential C residue cannot be providedby any alternative nucleotide (3). This degree of signal specificitydoes not rule out (nor does it implicate) any of the possibleinteracting partners listed above. However, because changing theessential C residue to the complementary G residue does not signaltermination despite maintaining the potential template-nascentstrand association, we favor the notion that the essential C residueprovides a signal in a way other than by its base pairing withthe nascent RNA strand. A model describing the process of reiterativetranscription during editing in the paramyxovirus Sendai virus(see below) has recently been proposed (11). A central themeof this model is that a region of the nascent strand immediatelyupstream of a slippery sequence provides a signal which modulatesreiterative transcription by making sequence-specific contactswith a site on the polymerase. It is possible that the role ofthe 3'-AUAC-5' tetranucleotide is to provide a signal within thenascent strand which somehow interacts with the VSV polymerasein a similarway.

Our detection of readthrough RNAs containing additional A residues indicates that a reiteratively transcribing polymerasecan resume processive transcription and transcribe the remainderof the template. Since the A/U group of templates exclusivelydirected synthesis of readthrough RNAs, the polymerase moleculesengaged in slippage must always return to the normal mode of transcription.The A tracts found in the readthrough RNAs generated by templateAUAA rarely exceeded 26 A residues in length (Fig. 6D) and werethus shorter than typical VSV mRNA poly(A) tails, which are between100 and 300 nucleotides long. Does this observation suggest thattermination of mRNA synthesis can occur only when polymerase slippagemakes an A tract that exceeds a certain critical length? We suggestthat while A-tract length may be an important factor in the terminationmechanism, it is not likely to be the only one, as many previousstudies have identified intervening A tracts in readthrough RNAsmuch larger than those of a typical VSV poly(A) tail (13, 14,28).

The ability of the VSV polymerase to regain template-dependent transcription after performing reiterative transcription onthe U7 tract, as described above, is strongly reminiscent of theediting activity by which many negative-strand viruses, most notablysimian virus 5, measles virus, and Sendai virus, have been shownto modulate transcription of their P genes (8, 37). Importantly,however, there are differences between these examples of nontemplatedtranscription. First, during P gene editing, the addition of nontemplatedG residues generally occurs in a controlled manner so that additionof a precise number of nucleotides is favored over all others.This contrasts with the findings of our present study, which revealedthat the number of nucleotide additions at the U₇ VSV slippagesite was distributed over a broad range. Second, unlike our findingsreported here, during paramyxovirus P gene editing, the insertedresidue (G) is templated by a nucleotide that is not within theslippage sequence itself but is located immediately downstream.Recent work involving Sendai virus has indicated that these twofeatures reflect differences in the template sequence rather thanfundamental differences in polymerase activity (11, 12). Thisresult, in combination with the finding that sequences immediatelyupstream of the U tract can regulate the reiterative transcriptionactivity of the Sendai virus and VSV polymerases, has revealeda strong mechanistic relationship between the process of mRNAediting and the polymerase slippage activity reported here. Aparallel may also be drawn between the VSV slippage activity andglycoprotein mRNA editing in Ebola virus, as both activities involveinsertion of A residues via slippage on a polyuridylate tract(29). Furthermore, the sequence responsible for the nucleotideadditions at the Ebola virus editing site strongly resembles anEbola virus gene end signal. Perhaps Ebola virus and other viruseswhich edit their mRNAs via a slippage mechanism have modifiedwhat once were termination signals in order to either increasethe coding flexibility of their genomes or reduce the attenuatingeffect of a genejunction.

Comparing the conserved gene end sequence of VSV to those of several other nonsegmented negative-stranded RNA viruses revealsthat sequences which precede the universal U tract share an A/U-richelement followed by a C residue that directly abuts the U tract.Because of this conservation, we suggest that many members ofthe family of nonsegmented negative-strand RNA viruses may utilizea common mechanism of not only polyadenylation but also the wayin which the termination process issignaled.

	ACKNOWLEDGMENTS

We thank members of the G. W. Wertz and L. A. Ball laboratories for helpful discussions during preparation of themanuscript.

This work was supported by PHS grant R37-A112464 from NIAID to G.W.W.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, BBRB 17/373, 845 19th St. South, University of Alabamaat Birmingham, Birmingham, AL 35294-2170. Phone: (205) 934 0877.Fax: (205) 934 1636. E-mail: gail_wertz{at}microbio.uab.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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8. Curran, J., R. Boeck, and D. Kolakofsky. 1991. The Sendai virus P gene expresses both an essential protein and an inhibitor of RNA synthesis by shuffling modules via mRNA editing. EMBO J. 10:3079-3085[Medline].

9. Emerson, S. U. 1982. Reconstitution studies detect a single polymerase entry site on the vesicular stomatitis virus genome. Cell 31:635-642[CrossRef][Medline].

10. Emerson, S. U., and R. R. Wagner. 1972. Dissociation and reconstitution of the transcriptase and template activities of vesicular stomatitis virus B and T virions. J. Virol. 10:297-309[Abstract/Free Full Text].

11. Hausmann, S., D. Garcin, C. Delenda, and D. Kolakofsky. 1999. The versatility of paramyxovirus RNA polymerase stuttering. J. Virol. 73:5568-5576[Abstract/Free Full Text].

12. Hausmann, S., D. Garcin, A. S. Morel, and D. Kolakofsky. 1999. Two nucleotides immediately upstream of the essential A6G3 slippery sequence modulate the pattern of G insertions during Sendai virus mRNA editing. J. Virol. 73:343-351[Abstract/Free Full Text].

13. Herman, R. C., S. Adler, R. A. Lazzarini, R. J. Colonno, A. K. Banerjee, and H. Westphal. 1978. Intervening polyadenylate sequences in RNA transcripts of vesicular stomatitis virus. Cell 15:587-596[CrossRef][Medline].

14. Herman, R. C., M. Schubert, J. D. Keene, and R. A. Lazzarini. 1980. Polycistronic vesicular stomatitis virus RNA transcripts. Proc. Natl. Acad. Sci. USA 77:4662-4665[Abstract/Free Full Text].

15. Hunt, D. M., E. F. Smith, and D. W. Buckley. 1984. Aberrant polyadenylation by a vesicular stomatitis virus mutant is due to an altered L protein. J. Virol. 52:515-521[Abstract/Free Full Text].

16. Hutchinson, K. L., R. C. Herman, and D. M. Hunt. 1992. Increased synthesis of polycistronic mRNA associated with increased polyadenylation by vesicular stomatitis virus. Virology 189:67-78[CrossRef][Medline].

17. Hwang, L. N., N. England, and A. K. Pattnaik. 1998. Polyadenylation of vesicular stomatitis virus mRNA dictates efficient transcription termination at the intercistronic gene junctions. J. Virol. 72:1805-1813[Abstract/Free Full Text].

18. Iverson, L. E., and J. K. Rose. 1981. Localized attenuation and discontinued synthesis during vesicular stomatitis virus transcription. Cell 23:477-484[CrossRef][Medline].

19. Leppert, M., L. Rittenhouse, J. Perrault, D. F. Summers, and D. Kolakofsky. 1979. Plus and minus strand leader RNAs in negative strand virus-infected cells. Cell 18:735-747[CrossRef][Medline].

20. Li, T., and A. K. Pattnaik. 1999. Overlapping signals for transcription and replication at the 3' terminus of the vesicular stomatitis virus genome. J. Virol. 73:444-452[Abstract/Free Full Text].

21. Macdonald, L. E., Y. Zhou, and W. T. McAllister. 1993. Termination and slippage by bacteriophage T7 RNA polymerase. J. Mol. Biol. 232:1030-1047[CrossRef][Medline].

22. Masters, P., and C. E. Samuel. 1984. Detection of in vivo synthesis of polycistronic mRNAs of vesicular stomatitis virus. Virology 134:277-286[CrossRef][Medline].

23. McGeoch, D. J. 1977. Structure of the gene N: gene NS intercistronic junction in the genome of vesicular stomatitis virus. Cell 17:673-681.

24. Moyer, S. A., S. Smallwood-Kentro, A. Haddad, and L. Prevec. 1991. Assembly and transcription of synthetic vesicular stomatitis virus nucleocapsids. J. Virol. 65:2170-2178[Abstract/Free Full Text].

25. Nudler, E., A. Mustaev, E. Lukhtanov, and A. Goldfarb. 1997. The RNA-DNA hybrid maintains the register of transcription by preventing backtracking of RNA polymerase. Cell 89:33-41[CrossRef][Medline].

26. Pattnaik, A. K., L. A. Ball, A. W. LeGrone, and G. W. Wertz. 1992. Infectious defective interfering particles of VSV from transcripts of a cDNA clone. Cell 69:1011-1020[CrossRef][Medline].

27. Rose, J. K. 1980. Complete intergenic and flanking gene sequences from the genome of vesicular stomatitis virus. Cell 19:415-421[CrossRef][Medline].

28. Rose, J. K., H. F. Lodish, and M. L. Brock. 1977. Giant heterogeneous polyadenylic acid on vesicular stomatitis virus mRNA synthesized in vitro in the presence of S-adenosylhomocysteine. J. Virol. 21:683-693[Abstract/Free Full Text].

29. Sanchez, A., S. G. Trappier, B. W. Mahy, C. J. Peters, and S. T. Nichol. 1996. The virion glycoproteins of Ebola viruses are encoded in two reading frames and are expressed through transcriptional editing. Proc. Natl. Acad. Sci. USA 93:3602-3607[Abstract/Free Full Text].

30. Schnell, M. J., L. Buonocore, M. A. Whitt, and J. K. Rose. 1996. The minimal conserved transcriptional stop-start signal promotes stable expression of a foreign gene in vesicular stomatitis virus. J. Virol. 70:2318-2323[Abstract].

31. Schubert, M., J. D. Keene, R. C. Herman, and R. A. Lazzarini. 1980. Site on the vesicular stomatitis virus genome specifying polyadenylation and the end of the L gene mRNA. J. Virol. 34:550-559[Abstract/Free Full Text].

32. Schubert, M., and R. A. Lazzarini. 1981. In vivo transcription of the 5'-terminal extracistronic region of vesicular stomatitis virus RNA. J. Virol. 38:256-262[Abstract/Free Full Text].

33. Smallwood, S., and S. A. Moyer. 1993. Promoter analysis of the vesicular stomatitis virus RNA polymerase. Virology 192:254-263[CrossRef][Medline].

34. Stillman, E. A., and M. A. Whitt. 1998. The length and sequence composition of vesicular stomatitis virus intergenic regions affect mRNA levels and the site of transcript initiation. J. Virol. 72:5565-5572[Abstract/Free Full Text].

35. Stillman, E. A., and M. A. Whitt. 1997. Mutational analyses of the intergenic dinucleotide and the transcriptional start sequence of vesicular stomatitis virus (VSV) define sequences required for efficient termination and initiation of VSV transcripts. J. Virol. 71:2127-2137[Abstract].

36. Stillman, E. A., and M. A. Whitt. 1999. Transcript initiation and 5'-end modifications are separable events during vesicular stomatitis virus transcription. J. Virol. 73:7199-7209[Abstract/Free Full Text].

37. Thomas, S. M., R. A. Lamb, and R. G. Paterson. 1988. Two mRNAs that differ by two nontemplated nucleotides encode the amino coterminal proteins P and V of the paramyxovirus SV5. Cell 54:891-902[CrossRef][Medline].

38. Villarreal, L. P., M. Breindl, and J. J. Holland. 1976. Determination of molar ratios of vesicular stomatitis virus induced species in BHK-21 cells. Biochemistry 15:1663-1667[CrossRef][Medline].

39. Volchkov, V. E., S. Becker, V. A. Volchkova, V. A. Ternovoj, A. N. Kotov, S. V. Netesov, and H. D. Klenk. 1995. GP mRNA of Ebola virus is edited by the Ebola virus polymerase and by T7 and vaccinia virus polymerases. Virology 214:421-430[CrossRef][Medline].

40. Whelan, S. P., J. N. Barr, and G. W. Wertz. 2000. Identification of a minimal size requirement for termination of vesicular stomatitis virus mRNA: implications for the mechanism of transcription. J. Virol. 74:8268-8276[Abstract/Free Full Text].

41. Whelan, S. P. J., and G. W. Wertz. 1999. Regulation of RNA synthesis by the genomic termini of vesicular stomatitis virus: identification of distinct sequences essential for transcription but not replication. J. Virol. 73:297-306[Abstract/Free Full Text].

42. Whelan, S. P. W., L. A. Ball, J. N. Barr, and G. W. Wertz. 1995. Efficient recovery of infectious vesicular stomatitis virus entirely from cDNA clones. Proc. Natl. Acad. Sci. USA 92:8388-8392[Abstract/Free Full Text].

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1.	Abraham, G., and A. K. Banerjee. 1976. Sequential transcription of the genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:1504-1508[Abstract/Free Full Text].
2.	Ball, L. A., and C. N. White. 1976. Order of transcription of genes of vesicular stomatitis virus. Proc. Natl. Acad. Sci. USA 73:442-446[Abstract/Free Full Text].
3.	Barr, J. N., S. P. Whelan, and G. W. Wertz. 1997. cis-acting signals involved in termination of vesicular stomatitis virus mRNA synthesis include the conserved AUAC and the U7 signal for polyadenylation. J. Virol. 71:8718-8725[Abstract].
4.	Barr, J. N., S. P. J. Whelan, and G. W. Wertz. 1997. Role of the intergenic dinucleotide in vesicular stomatitis virus RNA transcription. J. Virol. 71:1794-1801[Abstract].
5.	Bilsel, P. A., and S. T. Nichol. 1990. Polymerase errors accumulating during natural evolution of the glycoprotein gene of vesicular stomatitis virus Indiana serotype isolates. J. Virol. 64:4873-4883[Abstract/Free Full Text].
6.	Colonno, R. J., and A. K. Banerjee. 1978. Complete nucleotide sequence of the leader RNA synthesized in vitro by vesicular stomatitis virus. Cell 15:93-101[CrossRef][Medline].
7.	Colonno, R. J., and A. K. Banerjee. 1976. A unique RNA species involved in initiation of vesicular stomatitis virus RNA transcription in vitro. Cell 8:197-204[CrossRef][Medline].
8.	Curran, J., R. Boeck, and D. Kolakofsky. 1991. The Sendai virus P gene expresses both an essential protein and an inhibitor of RNA synthesis by shuffling modules via mRNA editing. EMBO J. 10:3079-3085[Medline].
9.	Emerson, S. U. 1982. Reconstitution studies detect a single polymerase entry site on the vesicular stomatitis virus genome. Cell 31:635-642[CrossRef][Medline].
10.	Emerson, S. U., and R. R. Wagner. 1972. Dissociation and reconstitution of the transcriptase and template activities of vesicular stomatitis virus B and T virions. J. Virol. 10:297-309[Abstract/Free Full Text].
11.	Hausmann, S., D. Garcin, C. Delenda, and D. Kolakofsky. 1999. The versatility of paramyxovirus RNA polymerase stuttering. J. Virol. 73:5568-5576[Abstract/Free Full Text].
12.	Hausmann, S., D. Garcin, A. S. Morel, and D. Kolakofsky. 1999. Two nucleotides immediately upstream of the essential A6G3 slippery sequence modulate the pattern of G insertions during Sendai virus mRNA editing. J. Virol. 73:343-351[Abstract/Free Full Text].
13.	Herman, R. C., S. Adler, R. A. Lazzarini, R. J. Colonno, A. K. Banerjee, and H. Westphal. 1978. Intervening polyadenylate sequences in RNA transcripts of vesicular stomatitis virus. Cell 15:587-596[CrossRef][Medline].
14.	Herman, R. C., M. Schubert, J. D. Keene, and R. A. Lazzarini. 1980. Polycistronic vesicular stomatitis virus RNA transcripts. Proc. Natl. Acad. Sci. USA 77:4662-4665[Abstract/Free Full Text].
15.	Hunt, D. M., E. F. Smith, and D. W. Buckley. 1984. Aberrant polyadenylation by a vesicular stomatitis virus mutant is due to an altered L protein. J. Virol. 52:515-521[Abstract/Free Full Text].
16.	Hutchinson, K. L., R. C. Herman, and D. M. Hunt. 1992. Increased synthesis of polycistronic mRNA associated with increased polyadenylation by vesicular stomatitis virus. Virology 189:67-78[CrossRef][Medline].
17.	Hwang, L. N., N. England, and A. K. Pattnaik. 1998. Polyadenylation of vesicular stomatitis virus mRNA dictates efficient transcription termination at the intercistronic gene junctions. J. Virol. 72:1805-1813[Abstract/Free Full Text].
18.	Iverson, L. E., and J. K. Rose. 1981. Localized attenuation and discontinued synthesis during vesicular stomatitis virus transcription. Cell 23:477-484[CrossRef][Medline].
19.	Leppert, M., L. Rittenhouse, J. Perrault, D. F. Summers, and D. Kolakofsky. 1979. Plus and minus strand leader RNAs in negative strand virus-infected cells. Cell 18:735-747[CrossRef][Medline].
20.	Li, T., and A. K. Pattnaik. 1999. Overlapping signals for transcription and replication at the 3' terminus of the vesicular stomatitis virus genome. J. Virol. 73:444-452[Abstract/Free Full Text].
21.	Macdonald, L. E., Y. Zhou, and W. T. McAllister. 1993. Termination and slippage by bacteriophage T7 RNA polymerase. J. Mol. Biol. 232:1030-1047[CrossRef][Medline].
22.	Masters, P., and C. E. Samuel. 1984. Detection of in vivo synthesis of polycistronic mRNAs of vesicular stomatitis virus. Virology 134:277-286[CrossRef][Medline].
23.	McGeoch, D. J. 1977. Structure of the gene N: gene NS intercistronic junction in the genome of vesicular stomatitis virus. Cell 17:673-681.
24.	Moyer, S. A., S. Smallwood-Kentro, A. Haddad, and L. Prevec. 1991. Assembly and transcription of synthetic vesicular stomatitis virus nucleocapsids. J. Virol. 65:2170-2178[Abstract/Free Full Text].
25.	Nudler, E., A. Mustaev, E. Lukhtanov, and A. Goldfarb. 1997. The RNA-DNA hybrid maintains the register of transcription by preventing backtracking of RNA polymerase. Cell 89:33-41[CrossRef][Medline].
26.	Pattnaik, A. K., L. A. Ball, A. W. LeGrone, and G. W. Wertz. 1992. Infectious defective interfering particles of VSV from transcripts of a cDNA clone. Cell 69:1011-1020[CrossRef][Medline].
27.	Rose, J. K. 1980. Complete intergenic and flanking gene sequences from the genome of vesicular stomatitis virus. Cell 19:415-421[CrossRef][Medline].
28.	Rose, J. K., H. F. Lodish, and M. L. Brock. 1977. Giant heterogeneous polyadenylic acid on vesicular stomatitis virus mRNA synthesized in vitro in the presence of S-adenosylhomocysteine. J. Virol. 21:683-693[Abstract/Free Full Text].
29.	Sanchez, A., S. G. Trappier, B. W. Mahy, C. J. Peters, and S. T. Nichol. 1996. The virion glycoproteins of Ebola viruses are encoded in two reading frames and are expressed through transcriptional editing. Proc. Natl. Acad. Sci. USA 93:3602-3607[Abstract/Free Full Text].
30.	Schnell, M. J., L. Buonocore, M. A. Whitt, and J. K. Rose. 1996. The minimal conserved transcriptional stop-start signal promotes stable expression of a foreign gene in vesicular stomatitis virus. J. Virol. 70:2318-2323[Abstract].
31.	Schubert, M., J. D. Keene, R. C. Herman, and R. A. Lazzarini. 1980. Site on the vesicular stomatitis virus genome specifying polyadenylation and the end of the L gene mRNA. J. Virol. 34:550-559[Abstract/Free Full Text].
32.	Schubert, M., and R. A. Lazzarini. 1981. In vivo transcription of the 5'-terminal extracistronic region of vesicular stomatitis virus RNA. J. Virol. 38:256-262[Abstract/Free Full Text].
33.	Smallwood, S., and S. A. Moyer. 1993. Promoter analysis of the vesicular stomatitis virus RNA polymerase. Virology 192:254-263[CrossRef][Medline].
34.	Stillman, E. A., and M. A. Whitt. 1998. The length and sequence composition of vesicular stomatitis virus intergenic regions affect mRNA levels and the site of transcript initiation. J. Virol. 72:5565-5572[Abstract/Free Full Text].
35.	Stillman, E. A., and M. A. Whitt. 1997. Mutational analyses of the intergenic dinucleotide and the transcriptional start sequence of vesicular stomatitis virus (VSV) define sequences required for efficient termination and initiation of VSV transcripts. J. Virol. 71:2127-2137[Abstract].
36.	Stillman, E. A., and M. A. Whitt. 1999. Transcript initiation and 5'-end modifications are separable events during vesicular stomatitis virus transcription. J. Virol. 73:7199-7209[Abstract/Free Full Text].
37.	Thomas, S. M., R. A. Lamb, and R. G. Paterson. 1988. Two mRNAs that differ by two nontemplated nucleotides encode the amino coterminal proteins P and V of the paramyxovirus SV5. Cell 54:891-902[CrossRef][Medline].
38.	Villarreal, L. P., M. Breindl, and J. J. Holland. 1976. Determination of molar ratios of vesicular stomatitis virus induced species in BHK-21 cells. Biochemistry 15:1663-1667[CrossRef][Medline].
39.	Volchkov, V. E., S. Becker, V. A. Volchkova, V. A. Ternovoj, A. N. Kotov, S. V. Netesov, and H. D. Klenk. 1995. GP mRNA of Ebola virus is edited by the Ebola virus polymerase and by T7 and vaccinia virus polymerases. Virology 214:421-430[CrossRef][Medline].
40.	Whelan, S. P., J. N. Barr, and G. W. Wertz. 2000. Identification of a minimal size requirement for termination of vesicular stomatitis virus mRNA: implications for the mechanism of transcription. J. Virol. 74:8268-8276[Abstract/Free Full Text].
41.	Whelan, S. P. J., and G. W. Wertz. 1999. Regulation of RNA synthesis by the genomic termini of vesicular stomatitis virus: identification of distinct sequences essential for transcription but not replication. J. Virol. 73:297-306[Abstract/Free Full Text].
42.	Whelan, S. P. W., L. A. Ball, J. N. Barr, and G. W. Wertz. 1995. Efficient recovery of infectious vesicular stomatitis virus entirely from cDNA clones. Proc. Natl. Acad. Sci. USA 92:8388-8392[Abstract/Free Full Text].