Requirement of Cysteines and Length of the Human Respiratory Syncytial Virus M2-1 Protein for Protein Function and Virus Viability

doi:10.1128/JVI.75.23.11328-11335.2001

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Journal of Virology, December 2001, p. 11328-11335, Vol. 75, No. 23
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.23.11328-11335.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Requirement of Cysteines and Length of the Human Respiratory Syncytial Virus M2-1 Protein for Protein Function and Virus Viability

Roderick S. Tang, Nick Nguyen, Xing Cheng, and Hong Jin^*

Aviron, Mountain View, California 94043

Received 20 July 2001/Accepted 13 September 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The M2-1 protein of human respiratory syncytial virus (hRSV) promotes processive RNA synthesis and readthrough at RSV genejunctions. It contains four highly conserved cysteines, threeof which are located in the Cys₃-His₁ motif at the N terminusof M2-1. Each of the four cysteines, at positions 7, 15, 21, and96, in the M2-1 protein of hRSV A2 strain was individually replacedby glycines. When tested in an RSV minigenome replicon systemusing $beta$ -galactosidase as a reporter gene, C7G, C15G, and C21Glocated in the Cys₃-His₁ motif showed a significant reductionin processive RNA synthesis compared to wild-type (wt) M2-1. C96G,which lies outside the Cys₃-His₁ motif, was fully functional insupporting processive RNA synthesis in vitro. Each of these cysteinesubstitutions was introduced into an infectious antigenomic cDNAclone derived from hRSV A2 strain. Except for C96G, which resultedin a viable virus, no viruses were recovered with mutations inthe Cys₃-His₁ motif. This indicates that the Cys₃-His₁ motif iscritical for M2-1 function and for RSV replication. The functionalrequirement of the C terminus of the M2-1 protein was examinedby engineering premature stop codons that caused truncations of17, 46, or 67 amino acids from the C terminus. A deletion of 46or 67 amino acids abolished the synthesis of full-length $beta$ -galactosidasemRNA and did not result in the recovery of viable viruses. However,a deletion of 17 amino acids from the C terminus of M2-1 reducedprocessive RNA synthesis in vitro and was well tolerated by RSV.Relocation of the M2-1 termination codon upstream of the M2-2initiation codons did not significantly affect the expressionof the M2-2 protein. Both rA2-Tr17 and rA2-C96G did not replicateas efficiently as wt rA2 in HEp-2 cells and was restricted inreplication in the respiratory tracts of cottonrats.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Human respiratory syncytial virus (hRSV) is an enveloped nonsegmented negative-strand RNA virus classified in the genus Pneumovirusof the family Paramyxoviridae (19). The genomic RNA of hRSVA2 strain is 15,222 nucleotides (nt) in length and encodes 11proteins from 10 genes in the following gene order: 3' NS1-NS2-N-P-M-SH-G-F-M2-L5'. Each gene transcription unit is flanked by highly conservedgene-start and gene-stop sequences and is monocistronic exceptfor the M2 gene, which encodes two proteins unique to pneumoviruses,M2-1 and M2-2 (6, 7, 16). As with other negative-strandRNA viruses, synthesis of viral RNA requires a genomic RNA encapsidatedwith the nucleoprotein (N) along with the virus-encoded phosphoprotein(P) and the large (L) polymerase protein (12, 29). In addition,the M2-1 protein is also required for synthesis of RSV RNA. TheM2-1 protein is an antiterminator that prevents premature terminationduring transcription (6, 10, 11) and enhances read-throughtranscription at gene junctions (13-15).

The M2 mRNAs of all pneumoviruses encode two open reading frames (ORFs) that overlap at a similar location but with differentoverlapping sequences (1, 8). The M2-1 of hRSV A2 strainutilizes approximately 70% of the entire coding capacity of theM2 mRNA. The second ORF is located towards the 3' end of the mRNAand overlaps M2-1 by 4, 8, or 10 amino acids, depending on theinitiation codon(s) used for translating M2-2. It has been proposedthat the translation of hRSV M2-2 occurs by a mechanism that involvesreverse translocation of ribosomes terminating at the first downstreamM2-1 stop codon (1). The M2-2 protein is dispensable for RSVreplication, and present data indicate that M2-2 is involved inregulating the switch between viral RNA transcription and replication(3, 17).

The M2-1 protein of hRSV A2 strain is 194 amino acids in length, with a molecular weight of approximately 22,150 (6, 7).It contains a Cys₃-His₁ motif in the N terminus from residues7 to 25 that is highly conserved among human, bovine, ovine, andmurine strains of pneumoviruses (1, 2, 29). Nuclear magneticresonance spectroscopy and zinc back-titration analyses of ananalogous Cys₃-His₁ motif found in the mammalian transcriptionfactor Nup475 indicate that the cysteines and histidine are involvedin coordinating zinc (26). Replacement of cysteine 7 and 15and histidine 25 by serine in this motif reduced the ability ofM2-1 protein to enhance transcription read-through and disruptedthe interaction between M2-1 and the N protein in transfectedcells (14). Mutations in the Cys₃-His₁ motif also affected thephosphorylation of the M2-1 protein (14). In addition to thethree cysteines in the Cys₃-His₁ motif, a fourth cysteine thatis highly conserved among the M2-1 proteins of pneumoviruses ispresent at position 96 (9). Cysteines are often involved inintra- and intermolecular disulfide bond formations that are importantfor the structural and functional integrity of proteins. For example,substitutions of glycines for cysteines in the $alpha$ trans-inducingfactor of herpes simplex virus resulted in temperature-sensitiveviruses (21). It is therefore of interest to know if the cysteineat position 96 of M2-1 is also important for protein functionand for virusreplication.

Sequence alignment of the M2-1 proteins from different pneumoviruses revealed heterogeneity in lengths at the C terminus ofthe protein (9). Among all known pneumovirus M2-1 proteins,the pneumovirus of mice (PVM) M2-1 is the shortest, differingby 17 amino acids from that of hRSV A2 strain (1, 9). Althougha functional motif has been located at the N terminus of M2-1,the requirements of the C terminus for protein function and virusreplication are notknown.

In this study we investigated the role of the cysteine residues in M2-1 function by replacing each of the four cysteines individuallywith glycine. The functional requirement of the C terminus ofM2-1 was also examined by deleting different numbers of aminoacids from the C terminal end of the protein. Alterations engineeredin the M2-1 protein were analyzed for their effects on processiveRNA synthesis in vitro. Furthermore, these changes were introducedinto an infectious antigenomic cDNA clone to evaluate their effectson virus recovery and virusreplication.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and viruses. Monolayers of Vero and HEp-2 cells were maintained in Dulbecco's modified Eagle medium supplemented with 10% fetal bovineserum. Modified vaccinia virus Ankara (MVA) expressing T7 RNApolymerase, MVA-T7, was provided by Bernard Moss (23, 28).MVA-T7 was propagated in CEK cells(SPAFAS).

Construction of RSV protein expression plasmids and minigenome. The protein expression plasmids that contained the N, P, or L gene under the control of a T7 promoter in pCITE2a vector (Novagen)were described previously (18). The M2-1 ORF was cloned intopCITE2a under the control of the T7 promoter (pM2-1). The cysteine-to-glycinechanges and tandem stop codons introduced into M2-1 are shownin Fig. 1. Mutations were introduced into pM2-1 using a QuikChangeSite-Directed Mutagenesis Kit (Stratagene), and the sequence ofthe entire M2-1 gene was confirmed by DNA sequence analysis.

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FIG. 1. (A) Cysteine scanning mutagenesis of the M2-1 gene. The underlined cysteine residues at position 7, 15, 21, and 96 were changed to glycine, and the mutants are denoted C96G, C15G, C21G, and C96G. (B) Three C-terminal-end truncations were engineered by the introduction of tandem stop codons, indicated by asterisks. Mutants with a truncation of 67, 46, or 17 amino acids are designated Tr67, Tr46, or Tr17.

RSV minigenome, pRSVLacZ, was engineered to encode a negative-sense $beta$ -galactosidase gene under the control of the T7 promoter.The $beta$ -galactosidase gene contains the RSV gene-start and gene-stopsequences flanked by the RSV trailer and leader sequences. TheRSV leader sequences are followed by the hepatitis delta virusribozyme and the T7 polymerase terminator sequences. The cDNAencoding $beta$ -galactosidase was amplified by PCR using a pair ofprimers containing the NheI and NsiI restriction enzyme sitesat its 5' and 3' ends, respectively. The NheI-to-NsiI restrictionfragment was then used to replace the chloramphenicol acetyltransferase(CAT) gene in the pRSVCAT minigenome through the XbaI and PstIrestriction sites. The NheI and NsiI restriction sites are compatiblewith the XbaI and PstI sites,respectively.

Construction of RSV antigenomic cDNA containing mutations in the M2-1 gene. To introduce M2-1 mutations into the full-length RSV antigenomic A2 cDNA clone, each mutation was first individually engineeredinto an RSV subclone, pET-S/B. pET-S/B contained a SacI-to-BamHIrestriction fragment bearing RSV sequences from nt 4477 to 8499,which included the entire M2 gene. The cysteine-to-glycine changesand the premature tandem stop codons were separately introducedinto pET-S/B by using a QuikChange Site-Directed Mutagenesis Kit(Stratagene). The SacI-to-BamHI restriction fragments containingthe M2-1 mutations were then used to replace the correspondingregion in pRSVC4G (18). pRSVC4G contained a C-to-G change inthe antigenomic sense in the RSV leader. All the M2-1 mutationsintroduced into the full-length antigenomic cDNA clones were confirmedby DNAsequencing.

Transfection and measurement of reporter gene expression. RSV RNA transcription and replication programmed by an RNA minigenome replicon (pRSVLacZ) was analyzed by transfection followinginfection with a recombinant vaccinia virus expressing T7 polymerase.Subconfluent HEp-2 cells were infected with MVA-T7 at a multiplicityof infection (MOI) of 1 PFU/cell, and virus was allowed to adsorbat room temperature for 1 h. The MVA-T7-infected cells were thentransfected with 0.2 µg of pN, 0.2 µg of pP, 0.1 µg of pL, 0.2µg of pRSVLac Z, and 0.3 µg of pM2-1 or its derivatives unlessotherwise indicated. The transfection was performed using lipofectACE(Life Technology) according to the manufacturer's protocol. Thetransfected cells were incubated at 33°C for 36 h, and cell extractswere prepared by lysis in cell permeabilization buffer that contained0.5% NP-40 and 20 mM $beta$ -mercaptoethanol. Cell lysates were clarifiedby centrifugation at 2,500 rpm for 5 min at 4°C in an Eppendorf5415C microcentrifuge and analyzed for $beta$ -galactosidase activityusing the substrate chlorophenol red- $beta$ -D-galactopyranoside (CPRG;Roche Molecular Biochemicals). Aliquots of the clarified lysateswere incubated with the detection buffer containing 5 mM CPRGin a microtiter plate at room temperature for various amountsof time. The change in optical density at 550 nm (OD₅₅₀) was measuredwith SPECTRAmax, a 340PC microplate spectrophotometer using SOFTmaxsoftware (Molecular Devices). The assay was shown to be linearlyresponsive up to an OD₅₅₀ of 3.0.

Recovery of infectious RSV bearing mutations in the M2-1 gene. Transfection and recovery of infectious RSV bearing mutations in the M2-1 gene were performed as described previously forrescue of recombinant RSV (5, 18). Briefly, subconfluentHEp-2 cells infected with MVA-T7 at 1 PFU/cell were transfectedwith 0.4 µg of pN, 0.4 µg of pP, 0.2 µg of pL, and 0.4 µg of anRSV antigenomic cDNA clone containing the engineered mutationsin the M2-1 gene. For some rescue experiments, 0.4 µg of pM2-1was also included in the transfection reaction. Following transfection,cells were incubated at 33°C for 3 days and the cell culture supernatantswere used to infect fresh Vero cells to amplify rescued viruses.The mutations introduced into the virus were confirmed by sequencingthe cDNA of the M2-1 gene obtained by reverse transcription (RT)-PCRof viral genomic RNA. Virus recovered from cDNA was plaque purifiedthree times and amplified in Vero cells. Virus stocks were stabilizedwith SPG (0.2 M sucrose, 3.8 mM KH₂ PO₄, 7.2 mM K₂HPO₄, and 5.4mM monosodium glutamate) and stored at $-$ 80°C.

Growth of viruses in cell culture. HEp-2 and Vero cells were used for multiple-cycle growth analyses. Cell monolayers in 6-cm-diameter dishes were infected withvirus at an MOI of 0.1 PFU/cell. After 1 h of adsorption, theinfected cells were washed twice with phosphate-buffered salineand incubated with 2 ml of OptiMEM at 35°C. At 24-h intervals180 µl of the culture supernatant was removed, stabilized withSPG and stored at $-$ 80°C prior to titration, and 180 µl of freshOptiMEM was added back to each well. For titration, Vero cellsin 12-well plates were infected with 10-fold serially dilutedvirus samples and overlaid with L-15 medium containing 1% methylcelluloseand 2% fetal bovine serum. After 6 days of incubation at 35°C,plaques were enumerated following immunostaining with a primarygoat anti-RSV antibody (Biogenesis) and a secondary rabbit anti-goatimmunoglobulin G conjugated with horseradish peroxidase. The amountof input viruses at the start of each experiment was verifiedby titration on Verocells.

RNA expression by Northern blot analyses. To examine RNA expression, total cellular RNA was prepared from virus-infected or DNA-transfected cells by using Trizol reagents(Life Technologies). The RNA was further extracted once with phenol-chloroformand precipitated with ethanol. RNA pellets were resuspended indiethyl pyrocarbonate-treated water and stored at $-$ 80°C. Equalamounts of total RNA were separated on 1% agarose gels containing1% formaldehyde and were transferred to nylon membranes (AmershamPharmacia Biotech) by using a Turboblotter apparatus (Schleicher& Schuell). The blots were hybridized with digoxigenin (DIG)-UTP-labeledriboprobes synthesized by in vitro transcription using a DIG RNAlabeling kit (Roche Molecular Biochemicals). Hybridization wascarried out at 68°C for 12 h in Express Hyb solution (Clontech).The blots were washed at 68°C twice with 2× SSC (1× SSC is 0.015M NaCl plus 0.015 M sodium citrate)-0.1% sodium dodecyl sulfate(SDS) followed by one wash with 1× SSC-0.1% SDS and a final washwith 0.1× SSC-0.1% SDS. Signals from the hybridized probes weredetected by using a DIG-Luminescent detection kit (Roche MolecularBiochemicals) and visualized by exposure to BioMax ML film(Kodak).

Analyses of RSV proteins by Western blotting and immunoprecipitation. For Western blot analyses, HEp-2 or Vero cells were infected with virus at an MOI of 0.1 PFU/cell and total cell lysates wereharvested at 48 h postinfection. Cells were disrupted in Laemmlibuffer (Bio-Rad), and equal amount of lysates were separated on15% polyacrylamide gels containing 0.1% SDS and were transferredto nylon membranes (Amersham Pharmacia Biotech). The blots wereincubated with guinea pig anti-M2-1 antibody (provided by JeyeshMeanger) or anti-N monoclonal antibody (provided by Jose Melero).The membrane was then incubated with a secondary antibody conjugatedwith horseradish peroxidase and the protein bands were developedusing the ECL substrate (Amersham Pharmacia Biotech). For immunoprecipitation,HEp-2 or Vero cells were infected at an MOI of 1 PFU/cell. At15 to 18 h postinfection, cells were incubated with Dulbecco'smodified Eagle medium deficient in methionine and cysteine (ICN)for 30 min and then were exposed to (100 µCi/ml) [³⁵S]methionine and [³⁵S]cysteine (Promix; Amersham Pharmacia Biotech) for 4 h. Immunoprecipitationof RSV-specific proteins from cytoplasmic extracts was performedwith goat anti-RSV A2 serum (Biogenesis), guinea pig anti-M2-1serum, or rabbit anti-M2-2 serum (17). Immunoprecipitated polypeptideswere separated on 17.5% polyacrylamide gels containing 0.1% SDSand 4 M urea or 15% polyacrylamide gels containing 0.1% SDS andwere detected byautoradiography.

Replication of M2-1 mutant viruses in cotton rats. Replication of M2-1 mutants was compared with the wt recombinant A2 RSV (rA2) in 4- to 6-week-old respiratory pathogen-freecotton rats (Sigmodon hispidus). Cotton rats in groups of fivewere inoculated with 10⁶ PFU of virus in 0.1 ml OptiMEM intranasally under light methoxyfluraneanesthesia. Four days after infection cotton rats were sacrificedby CO₂ asphyxiation and their nasal turbinates and lungs wereharvested. Tissues were homogenized and virus titers were determinedby plaque assay on Verocells.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Effects of M2-1 mutations on processive RNA transcription in vitro. To examine the effects of the engineered mutations on M2-1 function, mutant M2-1 proteins were analyzed for their abilityto promote processive RNA synthesis of a minigenome replicon supportedby the recombinant vaccinia virus-T7 expression system. The requirementof M2-1 protein for the synthesis of full-length RNA is greaterfor transcripts longer than 1.3 kb (10); therefore, the 3.1-kb $beta$ -galactosidase gene was selected as a reporter gene for thisanalysis. Transcription of the pRSVLacZ minigenome by T7 RNA polymerasegenerates an antisense $beta$ -galactosidase RNA. Production of the $beta$ -galactosidase mRNA and expression of the enzyme were dependenton M2-1 in addition to the RSV N, P, and L proteins. To determinethe amount of wt pM2-1 needed to produce $beta$ -galactosidase activitywithin the responsive range of the assay, MVA-T7-infected HEp-2cells were transfected with pRSVLacZ and plasmids expressing RSVN, P, and L proteins along with various amounts of wt pM2-1. Inthe absence of pM2-1, no $beta$ -galactosidase activity was detected(Fig. 2A). The level of $beta$ -galactosidase activity increased withincreasing amounts of pM2-1, and peak activity was observed at0.8 µg of pM2-1 plasmid. No further increase in $beta$ -galactosidaseactivity was detected with larger amounts of pM2-1. As shown inFig. 2A, transfection with 0.3 µg of wt pM2-1 expression plasmidproduced a signal within the responsive range of the $beta$ -galactosidaseassay and was used to compare the processive function of eachM2-1 mutant protein with that of wt M2-1 protein.

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FIG. 2. (A) Expression of $beta$ -galactosidase is dependent on the M2-1 protein. The indicated amount of pM2-1 expression plasmid was transfected into MVA-T7-infected HEp-2 cells together with 0.2 µg of pN, 0.2 µg of pP, 0.2 µg of pL, and 0.2 µg of pRSVLacZ minigenome. Thirty-six hours after transfection, the $beta$ -galactosidase activity was measured by incubating the cell lysates with 5 mM CPRG for 5 min. An average of three transfection experiments is shown. (B) Comparison of $beta$ -galactosidase activity from cells transfected with wt and mutant M2-1 expression plasmids. Cells were transfected with 0.3 µg of wt M2-1 plasmid, and the $beta$ -galactosidase activity following 30 min of incubation with CPRG is shown. (C) $beta$ -Galactosidase activities from cells transfected with wt, C96G, or Tr17 M2-1. The enzymatic activity was monitored for 45 min after incubation of the cell lysates with CPRG. The signal was linearly responsive up to an OD₅₅₀ of 3.0. (D) Northern blot of total RNA extracted from HEp-2 cells transfected with wt and mutant M2-1 expression plasmids. The blot was hybridized with a riboprobe specific for $beta$ -galactosidase mRNA. The LacZ antigenome is also indicated.

The level of $beta$ -galactosidase activity in the presence of different M2-1 mutants was compared to that for wt M2-1 (Fig. 2B).Substitutions of glycine for C7, C15, and C21 in the Cys₃-His₁motif and truncation of 67 or 46 amino acids from the C terminusof M2-1 (Tr67 and Tr46) drastically decreased the level of $beta$ -galactosidaseactivity. C7G, Tr67, and Tr46 reduced the amount of $beta$ -galactosidaseactivity to almost background levels. However, C15G and C21G didnot completely abolish the ability of M2-1 to support processiveRNA synthesis. $beta$ -galactosidase activity at a level of approximately20% that of wt M2-1 was produced in cells expressing C21G M2-1.C96G and Tr17 were able to support processive RNA synthesis ata level slightly less than that of wt M2-1. The $beta$ -galactosidaseactivity from cells expressing C96G and Tr17 was approximately80 and 60% that of wt M2-1, respectively. Figure 2C shows thatthe optical density reflecting the $beta$ -galactosidase enzymatic activityincreased linearly over a period of 45 min. Less $beta$ -galactosidaseactivity was detected in cells expressing C96G and Tr17 M2-1 comparedto that of wt M2-1, and the relative differences were similarthroughout the entire period of theassay.

The level of $beta$ -galactosidase RNA expression in transfected cells was further analyzed by Northern blot analysis (Fig. 2D). $beta$ -Galactosidase mRNAs were readily detected in cells expressingwt M2-1 protein. A negligible amount of full-length $beta$ -galactosidasemRNA was produced when pM2-1 was omitted. The $beta$ -galactosidasemRNA detected in cells transfected with C7G, Tr67, and Tr46 wascomparable to that obtained in the absence of wt M2-1. The amountof $beta$ -galactosidase mRNA detected in cells expressing C15G andC21G was less than 10% of that detected in cells expressing wtM2-1. The level of $beta$ -galactosidase RNA detected for C96G and Tr17M2-1 mutants was similar to that observed in wt pM2-1 transfectedcells. Comparable amounts of M2-1 mRNAs were detected in cellstransfected with wt pM2-1 and all its derivatives (data not shown).Thus, the level of $beta$ -galactosidase mRNA expression obtained byNorthern blotting was consistent with the observed enzymatic levelof $beta$ -galactosidase.

Recovery of recombinant RSV with mutations in M2-1. To examine the effect of the M2-1 mutations on virus replication, all the cysteine-to-glycine changes and premature stop codonswere introduced into the M2-1 gene of a full-length RSV antigenomiccDNA derived from the A2 strain. As expected from their in vitroactivity, recombinant viruses expressing C96G or Tr17 M2-1 wererecovered from HEp-2 cells. The wt pM2-1 expression plasmid wasnot required to rescue these recombinants. Multiple attempts weremade to recover the other M2-1 mutants, but no viruses were obtainedeven when the wt pM2-1 was included in the transfection reactions.Therefore, consistent with the in vitro minigenome analysis, mutationsthat significantly reduced the processivity function of M2-1 alsodisabled its ability to regenerate infectious virus. The two viableM2-1 RSV mutants recovered contained M2-1 mutations that did notseverely reduce the ability of M2-1 to support processive RNAsynthesis invitro.

Replication of rA2-C96G and rA2-Tr17 in HEp-2 and Vero cells. rA2-C96G and rA2-Tr17 were plaque purified and amplified in Vero cells, and the replication of these two viruses was comparedto that of wt rA2 in cell culture. In HEp-2 cells, rA2-C96G andrA2-Tr17 exhibited small plaque morphology, with plaque size reductionof approximately 30% relative to that of wt rA2. The plaque sizeof both viruses in Vero cells was similar to that of rA2. Theplaque forming efficiency of rA2-C96G and rA2-Tr17 at 33 and 39°Cwas examined in HEp-2 and Vero cells. No significant reductionin titer was observed for either virus at 39°C compared to thatat 33°C. The titer of rA2-C96G was reduced by approximately 10-foldat 39°C, but this difference was only observed in HEp-2cells.

Multiple-step replication cycles of rA2-C96G and rA2-Tr17 were performed in HEp-2 and Vero cells infected at an MOI of 0.1PFU/cell. As shown in Fig. 3, the growth kinetics of both rA2-C96Gand rA2-Tr17 were similar to that of rA2 in Vero cells, but bothviruses showed a reduction in peak titer of approximately 0.5log₁₀ relative to rA2. In HEp-2 cells, rA2-C96G and rA2-Tr17 reachedpeak titers that were reduced by 2.0 log₁₀ and 1.5 log_10, respectively,relative to wt rA2.

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FIG. 3. Multiple-step replication cycles in Vero and HEp-2 cells. Vero cells (top) or HEp-2 cells (bottom) were infected with rA2, rA2-Tr17, or rA2-C96G at an MOI of 0.1 PFU/cell. Aliquots of culture medium in duplicates were harvested at 24-h intervals, and the virus was quantitated by plaque assay on Vero cells.

Viral RNA expression. Viral mRNA accumulation and production of read-through transcripts generated by rA2-C96G and rA2-Tr17 were examined by Northernblotting. HEp-2 cells were infected with wt rA2, rA2-C96G, orrA2-Tr17 at 0.1 PFU/cell, and total cellular RNA was preparedat 24 and 48 h postinfection. The Northern blot was hybridizedwith an M2-specific riboprobe. A smaller amount of M2 mRNA wasdetected in rA2-C96G-infected cells than in wt rA2 and rA2-Tr17at 24 h postinfection (Fig. 4A). Both rA2-C96G and rA2-Tr17 producedless M2 mRNA than rA2 at 48 h postinfection. Transcription read-throughat the gene junction between the F and M2 genes (F-M2) is knownto be highly dependent on M2-1 and has been postulated to havea role in the regulation of M2-1 expression during RSV infection(13). Northern blotting was used to compare the amount of read-throughtranscripts at the F-M2 gene junction produced by the M2-1 mutantsand wt rA2. Total cellular RNA prepared at 48 h postinfectionwas probed with an F-specific riboprobe to detect the F mRNA andits read-through transcripts. Figure 4B shows the F mRNA, F-M2,and F-M2-L read-through transcripts generated by both M2-1 mutantsand wt rA2. Less F mRNA was detected for rA2-C96G, but the ratioof F to F-M2 or F-M2-L appeared to be similar to that of wt rA2and rA2-Tr17. Thus, M2-1 bearing a C96G change or a truncationof 17 amino acids did not show substantial alterations in theirability to support viral RNA transcription and read-through atgene junctions during RSV replication.

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FIG. 4. Northern blot analyses of viral RNA expression. HEp-2 cells were infected with rA2, rA2-Tr17, or rA2-C96G at an MOI of 0.1 PFU/ml. Total cellular RNA was extracted at 24 or 48 h postinfection (A) or at 48 h postinfection (B). The RNA blots were hybridized with DIG-UTP-labeled riboprobe specific to M2 (A) or F (B) mRNAs. The mRNA and read-through transcripts are indicated.

Viral protein expression of rA2-C96G and rA2-Tr17. Western blotting and immunoprecipitation were performed to compare the level of viral protein expression in cells infectedwith rA2-C96G, rA2-Tr17, or wt A2 at an MOI of 0.1 PFU/cell. Cellextracts were harvested at 48 h postinfection. Western blots wereprobed with anti-N and anti-M2-1 antibodies. As shown in Fig.5A, a similar level of viral protein expression was observed inVero cells infected with the three viruses. In HEp-2 cells, theamount of M2-1 and N was less than that in Vero cells, and M2-1of rA2-Tr17 was reduced by approximately twofold compared to thatof wt rA2. The M2-1 protein of rA2-Tr17 migrated faster on polyacrylamidegels, confirming the smaller size of the prematurely terminatedTr17 M2-1 protein. No detectable full-length M2-1 protein wasobserved in cells infected with rA2-Tr17, indicating that thetandem stop codons engineered in the M2-1 gene of rA2-Tr17 terminatedtranslation of M2-1 efficiently.

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FIG. 5. (A) Western blot of cell lysates infected with rA2, rA2-C96G, or rA2-Tr17. Total cellular proteins from infected cells were separated on 15% polyacrylamide gels containing 0.1% SDS, and the blots were hybridized separately with anti-M2-1 or anti-N antibodies. (B) Immunoprecipitation of labeled RSV polypeptides from infected HEp-2 or Vero cells. HEp-2 or Vero cells were infected with each virus as indicated, and the proteins were labeled with [³⁵S]methionine and [³⁵S]cysteine at 16 h postinfection. The labeled proteins were immunoprecipitated with anti-RSV or anti-M2-2 antibodies. The F1 protein from RSV-infected HEp-2 and Vero cells showed different gel mobilities, and less F1 was produced in rA2-Tr17-infected Vero cells in this particular experiment.

The introduction of the premature stop codons in the M2 gene of rA2-Tr17 abolished the translational overlap between M2-1and the downstream M2-2 ORF. Since this genetic alteration couldaffect the expression of M2-2, the amount of M2-2 protein producedby rA2-Tr17 was compared to that expressed by wt rA2. The electrophoreticpattern of RSV polypeptides immunoprecipitated from rA2-Tr17-and rA2-C96G-infected cells were similar to that of wt rA2 (Fig.5B), but the amount of these viral proteins was reduced relativeto that of rA2. It was noted that in this experiment, less F1protein was produced in rA2-Tr17-infected Vero cells, but thereduction of the F protein was not reproducible. M2-2 was detectedin Vero and HEp-2 cells infected with rA2-Tr17 and rA2-C96G. However,the amount of M2-2 expressed by both M2-1 mutants was also slightlylower than that of rA2. This might be due to the overall reductionin the level of virus replication exhibited by the M2-1 mutantviruses.

Electrophoretic mobility of C96G M2-1 protein from rA2-C96G-infected cells. Previously it was reported that multiple forms of M2-1 protein could be distinguished by differences in their electrophoreticmobilities on SDS-polyacrylamide gels (22). Recently it wasalso shown that both phosphorylated and nonphosphorylated formsof the M2-1 protein migrated with different gel mobilities underreducing conditions (14). Since cysteine residues are ofteninvolved in the formation of disulfide bonds, it is of interestto examine whether the C96G substitution in M2-1 resulted in anycovalent bond disruptions that would affect the conformation ofM2-1. The M2-1 proteins immunoprecipitated from rA2-C96G- or rA2-infectedcells were resolved on SDS-polyacrylamide gels following denaturationin the presence or absence of a reducing reagent (Fig. 6). Undernonreducing conditions three major bands, indicated as a, b, andc, were detected in wt rA2-infected cells. Two major species (a,b) with gel mobilities similar to those of wt M2-1 were detectedin rA-C96G-infected cells. A minor species, denoted c*, that migratedslower than wt M2-1 (c) was also detected in rA2-C96G-infectedcells. Under reducing conditions the M2-1 protein from rA2-C96G-infectedcells exhibited three major species similar to that of wt M2-1.In addition, a fourth species (d) was also observed for C96G M2-1under reducing condition (Fig. 6). The difference in the numberof major M2-1 species detected under reducing conditions indicatedthat replacement of cysteine at position 96 by glycine might havealtered the conformation of M2-1 and/or affected the modificationof the protein. The different electrophoretic migration of thethird species in the wt (c) and C96G (c*) M2-1 under nonreducingcondition suggested that C96 might be involved in the formationof covalent disulfide linkages that were disrupted by the glycinesubstitution. Although the C96G M2-1 protein showed distinct electrophoreticdifferences from the wt M2-1 protein, these differences did notappear to disrupt its interactions with N, since the N proteinwas readily coimmunoprecipitated with C96G M2-1 in rA2-C96G-infectedcells (data not shown).

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FIG. 6. Immunoprecipitation of the M2-1 proteins from infected cells. HEp-2 cells were infected with rA2, rA2T17, or rA2C96G at an MOI of 1 PFU/cell. The labeled M2-1 proteins were immunoprecipitated with anti-M2-1 antibody and denatured in the presence (right panel) or absence (left panel) of $beta$ -mercaptoethanol. Immunoprecipitated M2-1 proteins were resolved by SDS--15% polyacrylamide gel electrophoresis. The different forms of M2-1 on the SDS-polyacrylamide gel are indicated as a, b, c, c*, or d.

Genetic stability of rA2-C96G and rA2-Tr17. One of the rA2-Tr17 isolates was found to express a P protein with a retarded electrophoretic mobility (data not shown). DNAsequence analysis of the P gene from this viral isolate revealedthree alterations at nt 2482, 2627, and 2637. T2482C and T2637Cresulted in amino acid changes at position 46 from I to T andat position 98 from F to L. rA2-Tr17 with wt P or mutant P hadsimilar growth kinetics in vitro, and the significance of theseamino acid changes detected in P require further investigation.The propensity of C96G and the tandem stop codons to revert followingmultiple passages in Vero cells was then examined. DNA sequenceanalyses of M2-1 RT-PCR product from viruses that had undergonemultiple rounds of amplification in Vero cells did not revealany genetic reversions at position 96 of rA2-C96G or at the prematurestop codons of rA2-Tr17. This suggests that the C96G substitutionand the introduced premature stop codons (Tr17) are geneticallystable in tissueculture.

Replication of rA2-C96G and rA2-Tr17 in cotton rats. rA2-C96G and rA2-Tr17 were evaluated for their abilities to replicate in the respiratory tracts of cotton rats. Cotton ratswere inoculated with 10⁶ PFU of rA2, rA2-C96G, or rA2-Tr17 intranasally, and virus replicationin the lungs was measured by plaque assays on Vero cells. Thereplication of rA2-C96G was reduced by approximately 1.3 log₁₀compared to that of rA2. The replication of rA2-Tr17 was slightlymore restricted, and its titer in the lungs was reduced by about1.5 log₁₀ compared to that ofrA2.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The M2-1 protein of human RSV is an antiterminator that is required for processive RNA synthesis by the viral polymerase (5,6) and transcription read-through at gene junctions (13,15). These M2-1 functions may allow a greater number of polymerasemolecules to access genes distal from the polymerase entry siteand counteract RNA transcription attenuation during RSV replication.In this study we showed that the first three cysteines in theM2-1 protein were essential for supporting processive RNA synthesisin vitro, and no virus was recovered when any of these cysteineswere replaced with glycine. C96 located in the center of M2-1was not critical for virus replication. We also demonstrated thatthe last 17 amino acids could be removed from the C terminus ofM2-1 without severely impairing the function of M2-1 in vitroand invivo.

The cysteines in the highly conserved Cys₃-His₁ motif are predicted to coordinate zinc (26). When C7 or C15 of hRSV M2-1was changed to serine, the ability of M2-1 to promote transcriptionread-through at RSV gene junctions was drastically impaired (14).Disruption of the Cys₃-His₁ motif also altered the ratio betweenphosphorylated and nonphosphorylated forms of M2-1 and decreasedthe physical interaction between M2-1 and the N protein (14).M2-1 has also been demonstrated to bind RNA, and the RNA bindingdomain was mapped to a region between residues 59 and 85. Furthermore,the RNA binding capacity of M2-1 was found to be dependent onthe phosphorylation status of the protein (9). The effectsof the M2-1 mutations generated in this study were first examinedby an assay that measured M2-1-dependent processive RNA synthesisin vitro. Although replacement of the three cysteines in the Cys₃-His₁motif of M2-1 greatly reduced their ability to promote full-length $beta$ -galactosidase mRNA synthesis, the level of reduction for eachreplacement was different. C7G completely abolished the abilityof M2-1 to support production of full-length $beta$ -galactosidase mRNA,whereas C15G and C21G M2-1 generated full-length reporter geneRNA at a level 10 to 20% that of wt M2-1. This implied that thethree cysteines in the Cys₃-His₁ motif might play different structuralroles in the maintenance of M2-1 function. Even though a low levelof $beta$ -galactosidase RNA was detected for C15G and C21G, these mutationsdid not result in virus recovery, supporting the previous reportby Hardy and Wertz (14) that the Cys₃-His₁ motif is criticalfor M2-1 function. Replacement of the fourth highly conservedcysteine residue at position 96, which lies outside the conservedcysteine-rich motif, was not lethal to M2-1 function. The replicationof rA2-C96G, however, was less efficient in HEp-2 cells and wasrestricted in the respiratory tracts of cotton rats. M2-1 carryingthis mutation showed no detectable differences in their physicalinteraction with the N protein in rA2-C96G-infected cells. Asreported previously, several forms of M2-1 with distinct electrophoreticmobilities are present in RSV-infected cells (22). Under reducingconditions two major species of M2-1 proteins can be detected,and the slower migrating form was found to be phosphorylated (14).Although the M2-1 protein from rA2-C96G showed a band that migrateddifferently from wt M2-1, it exhibited two major species identicalto those of wt M2-1, of which the slowest migrating band likelyrepresented the phosphorylated form. This indicated that the C96Gchange did not affect the phosphorylation of M2-1. Under nonreducingconditions, C96G M2-1 also showed species with different gel mobilitiesfrom that of wt M2-1, suggesting that cysteine 96 is involvedin the formation of a disulfide bond. The disruption of this covalentbond may have altered the conformation of M2-1 and may accountfor the less efficient replication of rA2-C96G.

The M2-1 proteins of pneumoviruses are heterogeneous in their sequences and lengths at the C terminus, suggesting a less criticalrole for the C terminus. We made three M2-1 truncations by deleting67, 46, or 17 amino acids from the end of the C terminus. Theshortest truncation did not significantly disrupt M2-1 function,and an infectious virus bearing this truncation was obtained.Tr17 M2-1 coincided with the length of the PVM M2-1 protein. TheM2-1 protein of PVM was less efficient at supporting processiveRSV RNA synthesis than the hRSV M2-1 protein (unpublished results).In vitro analysis showed that the full-length $beta$ -galactosidasemRNA produced from cells expressing Tr17 M2-1 was reduced by about50 to 60% relative to that of wt M2-1. The recovered recombinantvirus, rA2-Tr17, replicated less efficiently in cell culture andin the lungs of cotton rats than wt rA2. These results indicatethat although the last 17 amino acids of M2-1 are dispensablefor virus growth, they are required for efficient virus replication.The mutations identified in the P gene of a rA2-Tr17 virus wereT-to-C changes, which probably resulted from biased hypermutation(4, 24). Sequencing of the P genes from several other rA2-Tr17isolates and from rA2-Tr17 after several in vitro passages didnot reveal any mutations in the P gene. This suggests that themutations in P are probably not compensatory mutations for overcomingthe defect in the M2-1 function of rA2-Tr17.

The ORF carrying M2-1 overlaps with that of M2-2, and the introduction of the premature stop codons in the M2-1 gene of rA2-Tr17abolished the overlap between the two M2 ORFs. Recently it wasshown that the location of the termination codon of M2-1 playeda crucial role in directing translation of M2-2 from the upstreaminitiation codons (1). It was found that when the initiationcodon of M2-2 was relocated downstream of the M2-1 terminationcodon in a synthetic template, expression of the second ORF wasabolished. We also constructed a synthetic DNA template in whichthe M2-2 ORF was replaced by the CAT gene. The expression of theCAT protein from the nonoverlapping structure was similar to thatof the overlapping structure (data not shown). The expressionof the M2-2 protein in rA2-Tr17-infected cells indicates thatribosomes are able to access the AUGs located downstream of theengineered premature stop codons to direct the translation ofM2-2. The difference between our result and that of Ahmadian etal. (1) might be due to differences in the sequences and/orstructures of the RNAs used in the two studies. Expression ofthe second ORF from a single mRNA has been shown to be less efficient,irrespective of whether the two ORFs overlapped or not (20).The overlapping structure between M2-1 and M2-2 might be importantfor regulating the level of M2-2 expression. M2-2 is a transcriptionalregulator involved in viral RNA replication and transcription.Removal of the M2-2 gene significantly reduced the amount of accumulatedgenomic and antigenomic RNA and resulted in a virus that replicatedless efficiently in HEp-2 cells and in cotton rats (3, 17).Since the M2-2 protein was expressed in rA2-Tr17-infected cellsand the minigenome analysis showed that Tr17 M2-1 had reducedprocessivity compared to that of wt M2-1, it is most likely thatthe less efficient replication of rA2-Tr17 is a result of theimpaired M2-1 function rather than any changes in M2-2 proteinexpression.

Previously, a single mutation (T7605C) in the gene start signal of the M2 gene was found to be a major determinant specifyingthe temperature-sensitive phenotype of a live attenuated RSV vaccinecandidate, cpts 248/404 (25). Phenotypic reversion of cpts 248/404was detected in virus isolated from immunized infants in a clinicalstudy (27). Our finding that both C96G and Tr17 mutations inthe M2-1 protein compromised the efficiency of RSV replicationin vitro and in vivo provides additional evidence that the M2-1protein has an essential role in RSVreplication.

	ACKNOWLEDGMENTS

We thank Aviron's animal facility for assistance with the cotton rat experiments, the tissue culture facility for supplyingcells, Robert Brazas for discussions and construction of the pRSVlacZminigenome, Helen Zhou and Mary Munoz for technical assistance,and George Kemble and Bin Lu for critical review of the manuscript.We are grateful to Jayesh Meanger and Jose Melero for providingantibodies.

This work was supported in part by National Institutes of Health SBIR grants (2R44A145267-01/02).

	FOOTNOTES

^* Corresponding author. Mailing address: Aviron, 297 N. Bernardo Ave., Mountain View, CA 94043. Phone: (650) 919-6587. Fax:(650) 919-6610/6611. E-mail: hjin{at}aviron.com.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ahmadian, G., J. S. Randhawa, and A. J. Easton. 2000. Expression of the ORF-2 protein of the human respiratory syncytial M2 gene is initiated by a ribosomal termination-dependent reinitiation mechanism. EMBO J. 19:2681-2689[CrossRef][Medline].

2. Alansari, H., and L. N. D. Potgieter. 1994. Molecular cloning and sequence analysis of the phosphoprotein, nucleocapsid protein, matrix protein and 22K (M2) protein of the ovine respiratory syncytial virus. J. Gen. Virol. 75:3597-3601[Abstract/Free Full Text].

3. Bermingham, A., and P. L. Collins. 1999. The M2-2 protein of human respiratory syncytial virus is a regulatory factor involved in the balance between RNA replication and transcription. Proc. Natl. Acad. Sci. USA 96:11259-11264[Abstract/Free Full Text].

4. Cattaneo, R. 1994. Biased (A $right-arrow$ I) hypermutation of animal RNA virus genomes. Curr. Opin. Genet. Dev. 4:895-900[CrossRef][Medline].

5. Collins, P. L., M. G. Hill, E. Camargo, H. Grosfeld, R. M. Chanock, and B. R. Murphy. 1995. Production of infectious human respiratory syncytial virus from cloned cDNA confirms an essential role for the transcription elongation factor from the 5' proximal open reading frame of the M2 mRNA in gene expression and provides a capability for vaccine development. Proc. Natl. Acad. Sci. USA 92:11563-11567[Abstract/Free Full Text].

6. Collins, P. L., M. G. Hill, J. Cristina, and H. Grosfeld. 1996. Transcription elongation factor of respiratory syncytial virus, a nonsegmented negative-strand RNA virus. Proc. Natl. Acad. Sci. USA 93:81-85[Abstract/Free Full Text].

7. Collins, P. L., M. G. Hill, and P. R. Johnson. 1990. The two open reading frames of the 22K mRNA of human respiratory syncytial virus: sequence comparison of antigenic subgroups A and B and expression in vitro. J. Gen. Virol. 71:3015-3020[Abstract/Free Full Text].

8. Collins, P. L., and G. W. Wertz. 1985. The envelope-associated 22K protein of human respiratory syncytial virus: nucleotide sequence of the mRNA and a related polytranscript. J. Virol. 54:65-71[Abstract/Free Full Text].

9. Cuesta, I., X. Geng, A. Asenjo, and N. Villanueva. 2000. Structural phosphoprotein M2-1 of the human respiratory syncytial virus is an RNA binding protein. J. Virol. 74:9858-9867[Abstract/Free Full Text].

10. Fearns, R., and P. L. Collins. 1999. Model for polymerase access to the overlapped L gene of respiratory syncytial virus. J. Virol. 73:388-397[Abstract/Free Full Text].

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12. Grosfeld, H., M. G. Hill, and P. L. Collins. 1995. RNA replication by respiratory syncytial virus (RSV) is directed by the N, P, and L protein; transcription also occurs under these conditions but requires RSV superinfection for efficient synthesis of full-length mRNA. J. Virol. 69:5677-5686[Abstract].

13. Hardy, R. W., S. B. Harmon, and G. W. Wertz. 1999. Diverse gene junctions of respiratory syncytial virus modulate the efficiency of transcription termination and respond differently to M2-mediated antitermination. J. Virol. 73:170-176[Abstract/Free Full Text].

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

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25. Whitehead, S. S., C. Y. Firestone, P. L. Collins, and B. R. Murphy. 1998. A single nucleotide substitution in the transcription start signal of the M2 gene of respiratory syncytial virus vaccine candidate cpts248/404 is the major determinant of the temperature-sensitive and attenuation phenotypes. Virology 247:232-239[CrossRef][Medline].

26. Worthington, M. T., B. T. Amann, D. Nathans, and J. M. Berg. 1996. Metal binding properties and secondary structure of the zinc-binding domain of Nup475. Proc. Natl. Acad. Sci. USA 93:13754-13759[Abstract/Free Full Text].

27. Wright, P. F., R. A. Karron, R. B. Belshe, J. Thompson, J. E. Crowe, Jr., T. G. Boyce, L. L. Halburnt, G. W. Reed, S. S. Whitehead, E. L. Anderson, A. E. Wittek, R. Casey, M. Eichelberger, B. Thumar, V. B. Randolph, S. A. Udem, R. M. Chanock, and B. R. Murphy. 2000. Evaluation of a live, cold-passaged, temperature-sensitive, respiratory syncytial virus vaccine candidate in infancy. J. Infect. Dis. 182:1331-1342[CrossRef][Medline].

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1.	Ahmadian, G., J. S. Randhawa, and A. J. Easton. 2000. Expression of the ORF-2 protein of the human respiratory syncytial M2 gene is initiated by a ribosomal termination-dependent reinitiation mechanism. EMBO J. 19:2681-2689[CrossRef][Medline].
2.	Alansari, H., and L. N. D. Potgieter. 1994. Molecular cloning and sequence analysis of the phosphoprotein, nucleocapsid protein, matrix protein and 22K (M2) protein of the ovine respiratory syncytial virus. J. Gen. Virol. 75:3597-3601[Abstract/Free Full Text].
3.	Bermingham, A., and P. L. Collins. 1999. The M2-2 protein of human respiratory syncytial virus is a regulatory factor involved in the balance between RNA replication and transcription. Proc. Natl. Acad. Sci. USA 96:11259-11264[Abstract/Free Full Text].
4.	Cattaneo, R. 1994. Biased (A $right-arrow$ I) hypermutation of animal RNA virus genomes. Curr. Opin. Genet. Dev. 4:895-900[CrossRef][Medline].
5.	Collins, P. L., M. G. Hill, E. Camargo, H. Grosfeld, R. M. Chanock, and B. R. Murphy. 1995. Production of infectious human respiratory syncytial virus from cloned cDNA confirms an essential role for the transcription elongation factor from the 5' proximal open reading frame of the M2 mRNA in gene expression and provides a capability for vaccine development. Proc. Natl. Acad. Sci. USA 92:11563-11567[Abstract/Free Full Text].
6.	Collins, P. L., M. G. Hill, J. Cristina, and H. Grosfeld. 1996. Transcription elongation factor of respiratory syncytial virus, a nonsegmented negative-strand RNA virus. Proc. Natl. Acad. Sci. USA 93:81-85[Abstract/Free Full Text].
7.	Collins, P. L., M. G. Hill, and P. R. Johnson. 1990. The two open reading frames of the 22K mRNA of human respiratory syncytial virus: sequence comparison of antigenic subgroups A and B and expression in vitro. J. Gen. Virol. 71:3015-3020[Abstract/Free Full Text].
8.	Collins, P. L., and G. W. Wertz. 1985. The envelope-associated 22K protein of human respiratory syncytial virus: nucleotide sequence of the mRNA and a related polytranscript. J. Virol. 54:65-71[Abstract/Free Full Text].
9.	Cuesta, I., X. Geng, A. Asenjo, and N. Villanueva. 2000. Structural phosphoprotein M2-1 of the human respiratory syncytial virus is an RNA binding protein. J. Virol. 74:9858-9867[Abstract/Free Full Text].
10.	Fearns, R., and P. L. Collins. 1999. Model for polymerase access to the overlapped L gene of respiratory syncytial virus. J. Virol. 73:388-397[Abstract/Free Full Text].
11.	Fearns, R., and P. L. Collins. 1999. Role of the M2-1 transcription antitermination protein of respiratory syncytial virus in sequential transcription. J. Virol. 73:5852-5864[Abstract/Free Full Text].
12.	Grosfeld, H., M. G. Hill, and P. L. Collins. 1995. RNA replication by respiratory syncytial virus (RSV) is directed by the N, P, and L protein; transcription also occurs under these conditions but requires RSV superinfection for efficient synthesis of full-length mRNA. J. Virol. 69:5677-5686[Abstract].
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