Generation of Bovine Respiratory Syncytial Virus (BRSV) from cDNA: BRSV NS2 Is Not Essential for Virus Replication in Tissue Culture, and the Human RSV Leader Region Acts as a Functional BRSV Genome Promoter

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Journal of Virology, January 1999, p. 251-259, Vol. 73, No. 1
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Generation of Bovine Respiratory Syncytial Virus (BRSV) from cDNA: BRSV NS2 Is Not Essential for Virus Replication in Tissue Culture, and the Human RSV Leader Region Acts as a Functional BRSV Genome Promoter

Ursula J. Buchholz, Stefan Finke, and Karl-Klaus Conzelmann^*

Department of Clinical Virology, Federal Research Center for Virus Diseases of Animals, D-72076 Tübingen, Germany

Received 2 July 1998/Accepted 8 October 1998

	ABSTRACT

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In order to generate recombinant bovine respiratory syncytial virus (BRSV), the genome of BRSV strain A51908, variant ATue51908,was cloned as cDNA. We provide here the sequence of the BRSV genomeends and of the entire L gene. This completes the sequence ofthe BRSV genome, which comprises a total of 15,140 nucleotides.To establish a vaccinia virus-free recovery system, a BHK-derivedcell line stably expressing T7 RNA polymerase was generated (BSRT7/5). Recombinant BRSV was reproducibly recovered from cDNA constructsafter T7 RNA polymerase-driven expression of antigenome senseRNA and of BRSV N, P, M2, and L proteins from transfected plasmids.Chimeric viruses in which the BRSV leader region was replacedby the human respiratory syncytial virus (HRSV) leader regionreplicated in cell culture as efficiently as their nonchimericcounterparts, demonstrating that all cis-acting sequences of theHRSV promoter are faithfully recognized by the BRSV polymerasecomplex. In addition, we report the successful recovery of a BRSVmutant lacking the complete NS2 gene, which encodes a nonstructuralprotein of unknown function. The NS2-deficient BRSV replicatedautonomously and could be passaged, demonstrating that NS2 isnot essential for virus replication in cell culture. However,growth of the mutant was considerably slower than and final infectioustiters were reduced by a factor of at least 10 compared to wild-typeBRSV, indicating that NS2 provides a supporting factor requiredfor full replicationcapacity.

	INTRODUCTION

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Bovine respiratory syncytial virus (BRSV) is a major etiological agent of respiratory tract disease in calves (43). Togetherwith human respiratory syncytial virus (HRSV) and pneumonia virusof mice, it belongs to the genus Pneumovirus within the familyParamyxoviridae (31). The BRSV genome encodes at least 10 proteinswhich are expressed by transcription of 10 mRNAs (24, 27).They include two nonstructural proteins (NS1 and NS2); four RNA-associatedproteins, namely, the nucleoprotein N, the phosphoprotein P, thelarge, catalytic subunit L of the RNA polymerase, and a transcriptionelongation factor encoded by the first of two overlapping openreading frames of the M2 gene (36); and three envelope-associatedproteins, namely, the fusion protein F, the attachment proteinG, and the small hydrophobic protein SH. Only a little is knownabout the function of the NS1 and NS2 genes, the presence of whichdistinguishes the members of the genus Pneumovirus from all otherparamyxoviruses. The NS1 protein of HRSV was recently found tostrongly inhibit transcription and replication in an HRSV minigenomesystem (1), whereas the function of NS2 is stillunclear.

As for all members of the order Mononegavirales, the genomic RNA of respiratory syncytial viruses is contained in a ribonucleoprotein(RNP) complex, in which it is tightly encapsidated by N and associatedwith P and L. Only RNA that is contained within an RNP complexmay serve as a template for the viral RNA polymerase (14, 46).Transcription and replication are directed by extragenic promoterswhich are located at the RNA ends. The genome promoter or leaderregion is located at the 3' end of the viral RNA and directs successivetranscription of a leader RNA (6) and free subgenomic mRNAsin the order 3'-le-NS1-NS2-N-P-M-SH-G-F-M2-L-5', as well as synthesisof a full-length antigenomic RNA. The latter appears to involvecotranscriptional encapsidation into the RNP complex. The 3' endof the antigenome RNA (the complement of the extragenic 5' regionof the genome, which is known as the "trailer") provides cis-actingsignals that solely direct replicative synthesis of full-lengthgenomicRNAs.

In recent years, protocols that allow intracellular reconstitution of RNP complexes of negative-strand RNA viruses entirelyfrom plasmid-derived components have been made available. Simultaneousexpression of full-length antigenome RNA and of individual RNP-associatedproteins resulted in the initiation of an infectious cycle andthe recovery of recombinant rhabdoviruses (23, 40, 45),paramyxoviruses (2, 4, 10, 13, 17, 18, 20, 32),and a bunyavirus (3). In the case of rhabdoviruses and mostparamyxoviruses, N, P, and L proteins were found to be sufficientto render full-length antigenome RNAs infectious. In the caseof HRSV, however, the M2 gene had to be expressed in additionto the N, P, and L proteins for successful recovery of recombinantHRSV (4).

We report here the cDNA cloning of the entire BRSV genome and the establishment of a system allowing genetic manipulationof BRSV in order to provide tools for experimental analysis ofpneumovirus molecular biology and for development of defined,attenuated vaccines. The integrity of the newly determined nucleotidesequences of the BRSV L gene and of the terminal BRSV promoterswas confirmed by successful recovery of recombinant BRSV. Interestingly,the HRSV genomic promoter was able to completely substitute forthe BRSV sequences. Moreover, the established vaccinia virus-freerecovery system allowed us to isolate considerably attenuatedvirus mutants and to provide direct evidence that the NS2 geneis not essential for BRSVreplication.

	MATERIALS AND METHODS

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Cells and virus. MDBK cells were infected at a multiplicity of infection (MOI) of 0.01 with cell culture supernatant of BRSV, strain A51908(American Type Culture Collection [ATCC]) (29). After 90 minof adsorption, the inoculum was removed and cells were incubatedat 37°C in minimal essential medium supplemented with 3% fetalcalf serum (FCS) in a 5% CO₂ atmosphere. After 8 days postinfection,when an extensive cytopathic effect (CPE) was observed, the mediumwas adjusted to 100 mM MgSO₄ and 50 mM HEPES (pH 7.5) (12),and the highly cell-associated virus was released by freezingand thawing. BRSV was also grown on BHK-21 cells (clone BSR T7/5),yielding lower titers. When propagated on BSR T7/5 cells, thevirus was harvested after 5 days postinfection, when the CPE wasmaximal. Titrations were carried out in duplicate in microwellplates by the limiting dilution method. To 0.1 ml of serial 10-foldvirus dilutions per well, 10⁴ BSR T7/5 cells were added in a 0.1-ml volume. After 48 h, cellswere fixed in 80% acetone. An indirect immunofluorescence assayusing a bovine serum specific to BRSV was done, and foci of infectedcells werecounted.

cDNA synthesis and cloning of genome ends. Five days postinfection, total RNA was prepared from MDBK cells infected with BRSV (RNeasy; Qiagen). cDNA clones coveringthe BRSV genome were generated by specifically primed preparativecDNA syntheses according to Gubler and Hofmann (15). The first-strandreaction was primed with an NS1 gene-specific synthetic oligonucleotideprimer (ATue51908 nucleotides [nt] 59 to 79) or with an oligonucleotidederived from the M2/L gene overlap (ATue51908 nt 8376 to 8393).Second-strand synthesis was done with a cDNA synthesis kit (Pharmacia);after NotI/EcoRI adapter ligation and size selection, the DNAwas cloned into Lambda ZAP II phages (Stratagene). Clones containingvirus cDNA were identified by plaque hybridization with [ $alpha$ -³²P]dCTP (3,000 Ci/mmol; ICN)-labeled (nick translation kit; Amersham)reverse transcription (RT)-PCR fragments derived from the N, G,or M2 gene, or restriction fragments from L gene cDNA clones.From positive phages, recombinant pBluescript SK was excised in vivo as recommended by the supplier. At leastthree independent cDNA clones were sequenced to generate the ATue51908consensus sequence. The NS1 and NS2 gene sequences (ATue51908nt 1 to 1146) and the terminal 1.4 kb of the L gene sequence (ATue51908nt 13701 to 15140) were verified by sequencing of cloned RT-PCRproducts.

The terminal sequences of genome and antigenome RNAs were determined by polyadenylation and subsequent RT-PCR. Briefly, 5µg of total RNA from infected cells was incubated for 30 min at37°C in a 50-µl reaction mix containing 5 units of poly(A) polymerase(Pharmacia Biotech), 40 mM Tris (pH 8.0), 10 mM MgCl₂, 2.5 mMMnCl₂, 250 mM NaCl, 250 µM ATP, and 50 µg of bovine serum albuminper ml. A one-tube RT-PCR containing a proofreading polymerase(Titan RT-PCR Kit; Boehringer Mannheim) was done on 1 µg of polyadenylatedRNA. For RT-PCR of the leader region, an oligo(dT) primer containinga HindIII site and a genome sense primer from the NS1 gene (ATue51908nt 306 to 286) were used. A fragment of about 300 bp was clonedinto pBluescript SK, and the leader consensus sequence was determined from six individualclones. To determine the trailer end, an additional RT-PCR fromthe polyadenylated RNA was done, assuming that polyadenylatedantigenome template was present. The RT-PCR was primed by theoligo(dT) primer and an antigenome sense oligonucleotide whichwas derived from the L gene/trailer consensus sequence previouslydetermined (ATue51908 nt 14980 to 15000). The expected fragmentof 160 bp was purified and cloned into pBluescript SKII prior to sequencing. All sequences were determined by an ABIPrism 377 automated sequencer; data were analyzed with the GeneticsComputer Group (GCG) Wisconsin Package, version 9.1 (GCG, Madison,Wis.).

Construction of BRSV full-length plasmids. As a backbone for the construction of transcription plasmids yielding antigenomic full-length RNA, the vector pX12 $Delta$ T, whichwas derived from pX8 $Delta$ T (40) by eliminating more restrictionsites from the multiple cloning site, was used. The plasmid containsthe 84 hepatitis delta virus (HDV) antigenome ribozyme sequencein the SmaI site, followed by a T7 RNA polymerase transcriptiontermination sequence in the BamHI site (40).

By a multiple-step cloning procedure, a synthetic T7 RNA polymerase promoter sequence followed by three nonviral G residuesand a synthetic leader sequence derived from HRSV strain A2 (nt1 to 44) (28), the BRSV NS1 and N genes, and the last 0.7 kbof the L gene and adjacent trailer were assembled in pX12 $Delta$ T sothat the last nucleotide of the trailer is directly followed bythe HDV ribozyme sequence. The NS1 noncoding region precedingthe translation start codon was modified to contain a syntheticNotI tag (see Results). Subsequently, the HRSV leader sequencewas replaced by the BRSV leader sequence by site-directed mutagenesis(22) in order to generate nonchimeric recombinants. Both theBRSV construct and the chimeric HRSV-BRSV construct were usedas backbone for the assembly of the complete BRSV genome fromcDNA. The first plasmids used for recovery of infectious recombinantvirus (rH/BRSV $Delta$ NS2, rBRSV $Delta$ NS2 [see Fig. 1]) were termed pH/BRSV $Delta$ NS2,encoding a chimera with HRSV leader sequence and a deletion ofthe complete NS2 gene, and pBRSV $Delta$ NS2, containing the homologousBRSV leadersequence.

The last step for generation of a recombinant full-length construct consisted of the insertion of the NS2 gene. The NS2 genewas obtained by RT-PCR, cloned in pBluescriptSK and sequenced, and transferred into the singular KpnI site ofthe full-length clones (ATue51908 nt 1,026) after restrictionof the PCR fragment with Acc65I and BanII and Klenow treatmentof all ends, resulting in a deletion of 4 nt (positions 510 to513) from the NS1 noncoding region following the NS1 translationstop codon. The resulting full-length plasmids were termed pBRSVand pH/BRSV, the latter containing the HRSV derived leader region.Figure 1 gives an overview of the four different recombinantsrecovered fromcDNA.

Construction of expression plasmids pN, pP, pL, and pM2. To allow cap-independent translation of mRNAs in T7 RNA polymerase-expressing cells, the encephalomyocarditis virus (EMCV)internal ribosomal entry site (IRES) (11) was cloned downstreamof the T7 RNA polymerase promoter of plasmid pT7T (9). PCRfragments in which the respective translation start codon is containedin an NcoI or AflIII restriction site were used to clone the openreading frame of the BRSV N (ATue51908 nt 1144 to 2605), P (ATue51908nt 2351 to 3249), M2 (ATue51908 nt 7523 to 8436), or L (ATue51908nt 8414 to 15140) gene into the NcoI site of the IRES specifyingthe translation start codon. Inserts generated by PCR were sequencedcompletely.

Establishment of a cell line stably expressing phage T7 RNA polymerase. To obtain a cell line stably expressing T7 RNA polymerase, 10⁶ BHK-21 cells (clone BSR-CL13) were transfected with 1 µg of pSC6-T7-NEOencoding the T7 RNA polymerase gene under control of the cytomegaloviruspromoter and the neomycin resistance gene (32) (kindly providedby M. Billeter). Resistant clones were selected after additionof geneticin (1 mg/ml) to the cell culture medium. T7 RNA polymeraseexpression of selected cell clones was monitored after transfectionof 5 µg of pT7T-N, which encodes the rabies virus N protein downstreamof the T7 RNA polymerase promoter (9). Two days after transfection,cells were stained with a fluorescein isothiocyanate conjugaterecognizing rabies virus N protein (Centocor) and analyzed byimmunofluorescence microscopy (not shown). After two further cloningsteps, a cell clone which constitutively expressed T7 RNA polymerase(BSR T7/5) was selected for further use. Even after 100 successivepassages (with every second passage involving geneticin selection),no decrease in T7 RNA polymerase-directed gene expression wasobserved in BSR T7/5cells.

Transfection experiments and recovery of recombinant BRSV (rBRSV). BSR T7/5 cells were grown overnight to 80% confluency in 32-mm-diameter dishes in Eagle's medium supplemented with 10% FCS.One hour before transfection, cells were washed twice with mediumwithout FCS. Cells were transfected with a plasmid mixture containing10 µg of full-length plasmid (pBRSV, pH/BRSV, pBRSV $Delta$ NS2, or pH/BRSV $Delta$ NS2),4 µg of pN, 4 µg of pP, 2 µg of pM2, and 2 µg of pL. Transfectionexperiments were carried out with a mammalian transfection kit(CaPO₄ transfection protocol; Stratagene). The transfection mediumwas removed at 4 h posttransfection; cells were washed and maintainedin Eagle's medium containing 3%FCS.

Five days after transfection, cells were split at a ratio of 1:3. Between 7 and 10 days posttransfection, a typical CPE wasobserved, yielding several foci per dish. The cells were splitevery 4 to 5 days, until between days 21 and 28 posttransfectiona total CPE was observed. The virus was released by freezing andthawing. Cellular debris was removed by pelleting at 800 × g,and the supernatant was used for production of high-titer materialin MDBK cells and for furtherexperiments.

Northern hybridization of viral RNA. Total RNA from BSR T7/5 cells was isolated at 2 to 5 days postinfection (RNeasy; Qiagen). The RNA was analyzed by denaturinggel electrophoresis (39), blotted onto nitrocellulose, cross-linkedto membranes by UV, and hybridized with DNA fragments labeled(nick translation kit; Amersham) with [ $alpha$ -³²P]dCTP (3,000 Ci/mmol; ICN). The N gene-specific probe was generatedby RT-PCR and tested for specificity by sequencing analysis beforeuse; the NS2-specific probe consisted of an AseI (ATue51908 nt574)/KpnI (ATue51908 nt 1026) fragment of a cloned and sequencedRT-PCR product which contains the complete NS2 open reading frame.Northern blots were exposed to Kodak X-Omat AR films at $-$ 70°Cwith an intensifyingscreen.

RT-PCR. To generate DNA probes for hybridization, for cloning of expression plasmids, and for RNA analysis of recombinant virus, RT-PCRwas done with avian myeloblastosis virus reverse transcriptase(Life Sciences) for first-strand synthesis, as described above,and a proofreading thermostable polymerase (Pfu; Stratagene) forPCR under conditions recommended by the supplier. The RNA of therecombinant viruses was analyzed by two sets of RT-PCR. The firstwas designed to demonstrate the synthetic NotI restriction sitefollowing the NS1 gene start. First-strand primers were selectedto hybridize to the 3' end of genomic RNA. The reverse primer(ATue51908 nt 306 to 286) was derived from the NS1 gene sequence.The second PCR was designed to demonstrate the absence or presenceof the NS2 gene. First-strand synthesis was done with the sameset of leader-specific primers, whereas a primer derived fromthe N gene sequence (ATue51908 nt 1165 to 1146) served as reverseprimer.

Nucleotide sequence accession number. The nucleotide sequence of BRSV strain ATue51908 has been deposited in the GenBank database under accession no. AF092942.

	RESULTS

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cDNA cloning and sequence analysis of BRSV strain ATue51908. We generated cDNA clones covering the complete genome of BRSV strain A51908, as obtained from the ATCC, after 12 passagesin MDBK cells. The sequence of the 3' half of the BRSV genomewas available, covering nine genes from the NS1 gene to the M2-Lgene overlap (25, 26, 30, 37, 38, 47, 48) (see Fig.1). Two primers were selected for specific priming of first-strandcDNA synthesis, the first hybridizing to the 3' proximal NS1 noncodingregion and the second hybridizing to the M2-L gene overlap. TotalRNA of BRSV-infected cells was used as starting material. Virus-specificcDNA clones were detected by hybridization with PCR probes derivedfrom the N, G, and M2 genes. Each probe was tested for specificityby sequence analysis and by hybridization with virus RNA beforeuse. Clones covering the entire L gene were obtained by genomewalking. Besides the correctly primed cDNA clones, we found aconsiderable amount of BRSV-specific clones that were random primed,together covering the entire genome except for the NS2 gene. Aconsensus sequence was derived from at least three independentcDNA clones. The last 1.4 kb of the genomic sequence and the NS1and NS2 gene sequences were, in addition, confirmed by sequencingof cloned RT-PCR fragments. In this case, at least six differentPCR clones were analyzed to generate a consensussequence.

Nucleotides 46 to 8454 of the consensus sequence, spanning the NS1, NS2, N, P, M, SH, G, F, and M2 genes, were compared tothe previously published sequences of BRSV strain A51908 (GenBankaccession no. U15937 [NS1], U15938 [NS2], M35076 [N],M93127 [P], D01012 [M and SH], and M82816 [F and M2][26, 48]), revealing considerable divergence. The total sequenceidentity was found to be 96.2%, owing to 319 differences and 10gaps in 8,454 nt. For the NS1, NS2, N, P, M, F, and M2 genes,sequence identities were in the range of 95 to 98%, and the aminoacid identity ranged between 100 and 97%. Both the SH and theG genes exhibited nucleotide identity of merely 93% with the publishedA51908 sequences. In the deduced SH and G proteins, only 86 and88% of the amino acids are identical, respectively. Together,the predicted amino acid sequences of the nine genes contain 97differences compared to the A51908 sequence, over a total of 2,263amino acids. Since the sequence data obtained differed substantiallyfrom the published A51908 sequence, we designated our startingvirus BRSV strain ATue51908. The total sequence of BRSV strainATue51908 (GenBank accession no. AF092942) comprises 15,140nt and codes for 10 mRNAs (Fig. 1). As described for other strains,the G and M2 mRNAs each contain two open reading frames.

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FIG. 1. Schematic presentation of the BRSV ATue51908 genome (drawn to scale). The locations of transcripts (shaded bars) and protein-encoding frames (open bars) are shown relative to the viral RNA (vRNA) (solid bar). In the enlargements, the organizations of recombinant viruses and ATue51908 are compared. The 3'-terminal 45-nt BRSV leader regions are marked by horizontal stripes, and the 44-nt HRSV A2 leader regions are marked by vertical stripes. Genetic tags (NotI) and nucleotide deletions in the NS1 noncoding regions (shaded) of the recombinant viruses are indicated. The relative positions of corresponding nucleotides are given for the gene starts of NS1, NS2, and N and nucleotides flanking the NS2 deletion. The overall lengths of the vRNAs are shown on the right.

Sequence of the ATue51908 L gene. Until now, the sequence of the largest BRSV gene coding for the catalytic subunit of the viral RNP-dependent RNA polymerase(L) was not available. The BRSV L gene has a length of 6,573 nt,including the gene start signal (5'-GGACAAAA-3' [DNA positivestrand]) and the transcription stop and polyadenylation signal(5'-AGTTATTTAAAAA-3' [positive strand]). The first ATG locatedin a favorable context for initiation of translation is partiallycontained in the gene start signal (5'-GGACAAAATG-3'), resultingin an extremely short 5' noncoding region of 7 nt. The translationstop codon, TAA, is followed by a noncoding region of 64 nt andthe transcription stop/polyadenylation signal. The predicted openreading frame codes for a protein of 2,162 amino acids. No additionalopen reading frames longer than 30 amino acids wereidentified.

Compared to the L gene of HRSV strain A2 (41), the BRSV L gene has identity of 77% and encodes a protein with amino acididentity of 84%. The L proteins of BRSV, HRSV, and turkey rhinotracheitisvirus (TRTV) (34) share an amino-terminal extension of about20 amino acids and a carboxy-terminal truncation of about 100amino acids, compared to L proteins of other nonsegmented negative-strandRNA viruses. This feature therefore appears to be common in thePneumovirinaesubfamily.

Sequence analysis of the BRSV leader and trailer regions. The leader region of BRSV (Fig. 2A) is 45 nt in length, 1 nt longer than that of HRSV A2 (28). The terminal regions arehighly conserved. Compared to HRSV, the first 17 nt are identicaland the first 28 nt contain two differences. Overall, the twoRSV leader regions have identity of 82%. Alignment of the BRSVand HRSV leader regions to that of TRTV (33) revealed identitiesof 61 and 67%, respectively.

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FIG. 2. Alignment of the BRSV ATue51908 3' leader region (A) and 5' trailer (B) sequences with those from other pneumoviruses. The DNA sequences are shown in 3'-to-5' viral RNA sense. For HRSV strain A2 (28) and TRTV (33), only deviations from the ATue51908 sequence are indicated. Gaps are represented by dots, and the start signal of the first gene (NS1 in BRSV and HRSV, N in TRTV) and the L gene end signal are underlined. Numbering of the trailer sequences starts with the first nucleotide downstream of the L gene transcription stop signal. (C) Alignment of the NS1 noncoding region of the recombinant BRSVs containing the NotI tag (boxed) with the ATue51908 consensus sequence and the published A51908 sequence. The sequences are shown as DNA positive strands. Only nucleotides differing from the recombinant sequence are indicated. Gaps are indicated by dots, and the NS1 gene start signal and translation start codon are underlined.

The 5' extragenic region of the BRSV genome (Fig. 2B) is composed of 161 nt, which is 6 nt longer than the HRSV A2 trailerregion (28). This is thus far the longest trailer sequence ofa member of the Paramyxoviridae family. The BRSV leader and trailerregions themselves exhibit a terminal complementarity of the extreme11 nt which is interrupted at position 4, as is also found inTRTV. The 5'-terminal 14 nt of BRSV and HRSV are identical, andthe 5'-terminal 25 nt contain only one different nucleotide. TheL-proximal two-thirds of the trailer regions show a very low degreeof homology, and the overall identity is 51%. The TRTV trailerregion (33), which is composed of only 40 nt, is more similarto the aligned region of HRSV than of BRSV (60 and 50% identity,respectively).

Construction of full-length BRSV cDNA clones. A cDNA copy of the BRSV genome was assembled in pX12 $Delta$ T downstream of a T7 RNA polymerase promoter such that antigenomic RNAwould be transcribed. Three G residues were introduced betweenthe promoter and the leader sequence to facilitate initiationof transcription. It was previously shown that additional nucleotidesat the 5' ends of HRSV genomes do not interfere with encapsidationand replication (35). To achieve correct cleavage of the RNAtranscript at the 3' end of the antigenome-like RNA, the HDV antigenomeribozyme sequence was joined directly to the last nucleotide ofthe trailer sequence (40).

At first, an NS2 deletion mutant was assembled in a plasmid containing the HRSV A2 leader region (nt 1 to 44) (28) insteadof the BRSV leader region and in which the NS1 gene end signal,the NS2 gene start signal, and the complete NS2 coding region(514 nt) are absent (rH/BRSV $Delta$ NS2 [Fig. 1]). Thus, the NS1 translationstop codon is followed by the gene end signal derived from theNS2 gene. Subsequently, an RT-PCR-generated NS2 gene sequencewas introduced into the NS2-deficient cDNA to generate a nondeficient,chimeric full-length genome (rH/BRSV [Fig. 1]). Due to the cloningprocedure, 4 nt from the wild-type noncoding sequence betweenthe NS1 translation stop codon and the NS1 gene end signal (nt510 to 513) were deleted. To finally replace the HRSV leader sequenceby the original BRSV leader sequence, site-directed mutagenesiswas done, giving rise to rBRSV $Delta$ NS2 and rBRSV (for details, seeMaterials andMethods).

All four cDNA constructs contain three common differences from the standard ATue51908 sequence: a 16-nt difference, involvingdeletion of one nucleotide, in the NS1 5' noncoding region, creatinga singular NotI site and allowing easy discrimination of recombinantvirus and wild-type ATue51908 virus (Fig. 2C), as well as twosingle nucleotide exchanges which are derived from one of thecDNA clones used for cloning (pL23). One of the exchanges is locatedin the BRSV trailer sequence (nt 15049, T to C) and the otherin the L coding sequence (nt 14312, A to C), resulting in an aminoacid change from isoleucine to leucine. Overall, the genome ofthe full-length BRSV recombinant is 5 nt shorter than the standardATue51908 virus genome, and the chimeric rH/BRSV sequence is 6nt shorter, due to the shorter HRSV leader. The genomes of theNS2 deletion mutants rBRSV $Delta$ NS2 and rH/BRSV $Delta$ NS2 are lacking 514internal nucleotides (Fig. 1).

Recovery of infectious BRSV from cDNA in a vaccinia virus-free cell system. Most systems for recovery of negative-strand RNA viruses make use of vaccinia helper virus providing T7 RNA polymerase forintracellular transcription of full-length RNAs and expressionof support proteins. However, to prevent possible interferencewith the notoriously very slow BRSV replication or virus assemblyand to avoid the necessity of separating vaccinia virus from BRSV,we decided to establish a vaccinia virus-free system. A cell linewhich stably expresses phage T7 RNA polymerase (BSR T7/5) wasgenerated by transfection of BHK-21 cells, clone BSR-CL13, witha plasmid expressing phage T7 RNA polymerase under control ofthe cytomegalovirus promoter (pSC6-T7-NEO, kindly provided byM. Billeter). BSR T7/5 cells were transfected with plasmids expressingantigenomic BRSV RNA and support plasmids expressing the BRSVN, P, L, and M2 proteins. The support plasmids contained the consensussequence of the respective ATue51908 open reading frame, downstreamof the ECMV IRES sequence, to allow cap-independent translation.Five days after transfection, cells were split in a 1:3 ratio.Between days 7 and 10 after transfection, a typical CPE was observed,in the form of several foci of fusing cells per dish. When anyof the support plasmids was omitted, no foci wereobserved.

All transfection experiments were done in quadruplicate and repeated at least three times. Each of the four different full-lengthconstructs yielded recombinant virus in all dishes. The cellswere split every 4 to 5 days, and the recovered virus was releasedby freezing and thawing when the CPE was maximal. Clarified supernatantwas used for three rounds of amplification in the case of thefull-length recombinant. In order to amplify the NS2 deletionmutant, at least five passages were necessary to produce stockmaterial suitable for furthercharacterizations.

Identification of genetic tags and transcription analysis of recombinant virus. Genetic tags were used to confirm the identity of the recombinant viruses. Total RNA of virus-infected BSR T7/5 cells wasisolated when the CPE was maximal, and RT-PCR was performed. Oneassay was done to demonstrate the novel NotI restriction sitecontained in the NS1 5' noncoding region of all recombinant viruses.Primers LeBRSV or LeH/BRSV and NS1r, which are specific for theleader regions and the NS1 gene, respectively, were used to amplifya 300-bp fragment which was then digested with NotI. The RT-PCRproducts obtained from recombinant viruses were cleaved by NotI,whereas the fragment obtained from standard ATue51908 virus wasnot (Fig. 3). A second RT-PCR with the leader-specific primerand the primer Nr, specific for the N gene, was designed to revealthe absence or presence of the NS2 gene. A PCR product of 1.2kb was obtained in the case of standard ATue51908 virus or offull-length recombinant viruses (Fig. 4). In the case of rBRSV $Delta$ NS2and rH/BRSV $Delta$ NS2, a fragment of about 0.7 kb was amplified by thesame primers, demonstrating the deletion of the NS2 gene. No PCRproduct was detected when the RT step was omitted (not shown),demonstrating that the PCR products originate from viral RNA ratherthan from plasmid contaminations.

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FIG. 3. Demonstration of the NotI tag in the genome RNA of recombinant BRSVs. RT-PCR was performed on total RNA of BSR T7/5 cells infected with standard BRSV ATue51908 or with recombinant virus by using positive-sense primers annealing to the genome 3' ends and a negative-sense primer binding in the NS1 gene. No PCR product was detected when the RT step was omitted. Digestion with NotI of the 324-bp (calculated size) RT-PCR product originating from recombinant viruses yielded two bands of calculated sizes of 82 and 242 bp, whereas the RT-PCR product from standard BRSV strain ATue51908 was not cleaved.

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FIG. 4. Demonstration of NS2 gene deletion by RT-PCR. Total RNA of BSR T7/5 cells infected with standard BRSV ATue51908 or with recombinant virus was used for RT-PCR with a positive-sense primer hybridizing to the 3' end of the BRSV genome RNA and a negative-sense primer binding in the N gene. Products from full-length recombinants and wild-type virus yielded a product of 1,179 bp (calculated size) spanning the NS2 gene, whereas deletion mutants gave rise to a 666-bp (calculated) fragment, reflecting the 513-nt deletion. No PCR product was detected when the RT step was omitted.

In order to demonstrate transcripts from the recombinant viruses and from standard ATue51908, RNA of infected cells was analyzedby Northern hybridization. Total cellular RNA was isolated 5 daysafter infection of BSR T7/5 cells at an MOI of 0.01. After hybridizationwith an N-specific probe, genome RNAs and monocistronic N mRNAswere detected in cells infected with the recombinant BRSVs andstandard ATue51908, demonstrating efficient transcription andreplication of the recombinant BRSVs (Fig. 5). In addition, aprominent band representing bicistronic N/P readthrough mRNA waspresent in all lanes. RNA from cells infected with the NS2 deletionmutants did not hybridize with an NS2 probe, whereas a prominentband corresponding to NS2 mRNA was present in cells infected withATue51908 or the full-length recombinants (Fig. 5). These resultsagain confirmed the absence of the complete NS2 gene in the genomeof deletion mutants, as well as the absence of contaminating helpervirus. The NS2 deletion mutants thus replicate autonomously incell culture.

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FIG. 5. Demonstration of virus transcripts by Northern hybridization. Total RNA of BSR T7/5 cells infected with rBRSV or standard ATue51908 was isolated 2 to 4 days after infection and separated on a 2% denaturing agarose gel. The blot was hybridized with PCR-derived probes specific for the BRSV N gene (nt 1429 to 2277) (A) and for the NS2 gene (nt 574 to 1026) (B). Transcripts corresponding to N mRNA (vRNA), bicistronic N/P readthrough transcripts, and NS2 mRNA are indicated.

Recombinant viruses lacking the NS2 gene are attenuated in cell culture. Growth characteristics of recombinant BRSV were studied with both the BHK-derived BSR T7/5 cell line and MDBK cells. The twofull-length recombinants did not differ from standard ATue51908virus in their final titers of infectious virus nor in their growthkinetics or phenotype. In MDBK cells, ATue51908 and the full-lengthrecombinants yielded maximal titers of 10⁶ PFU/ml after 8 days of infection at an MOI of 0.01, while inBSR T7/5 cells maximum titers of 10⁵ PFU/ml were achieved at 4 days after infection at the same MOI.The chimeric viruses containing the HRSV leader region did notdiffer in any respect from the recombinants containing the autologousBRSV leader sequence. Compared to the full-length viruses, theNS2 deletion mutants showed slower growth and reduced final titersin both BSR T7/5 and MDBK cells. In BSR T7/5 cells, a similartype of CPE, consisting of large syncytia detaching from the monolayer,developed after infection with both full-length and NS2-deficientviruses (Fig. 6A). When grown on MDBK cells, the full-length virusescaused typical foci of enlarged cells, indistinguishable fromstandard ATue51908 virus foci (Fig. 6B). The NS2 deletion mutants,however, yielded only small pinpoint foci in MDBK monolayers,consisting of a small number of infected cells (Fig. 6B). Dueto their very slow growth in MDBK, cells had to be split everythree days in a 1:3 ratio to keep the infection going on. At 15days after infection of MDBK cells at an MOI of 0.01, antigenwas detected in less than 60% of cells. In contrast, in the caseof standard ATue51908 or of full-length recombinant virus, itwas not possible to split MDBK cells infected with an MOI of 0.01more than once due to an extensive CPE. When BSR T7/5 cells wereinfected with the NS2 deletion mutants at an MOI of 0.01, CPEwas maximal at 5 days after infection. In these cultures, antigenwas detected in more than 80% of cells. Still, compared to full-lengthvirus, maximum titers of the NS2 deletion mutants were 10-foldlower in both cell lines, with maximum titers reaching 10⁴ PFU per ml in BSR T7/5 cells at 5 days after infection and 10⁵ PFU per ml in MDBK cells at 15 days after infection and fourpassages of infected cells. These features demonstrate that theNS2 gene is nonessential, though in its absence the replicationcapacity of BRSV is reduced and the CPE in MDBK cells is lesspronounced.

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FIG. 6. CPE of recombinant BRSVs in BSR T7/5 cells (A) and MDBK cells (B). (A) In BSR T7/5 cultures, all recombinants induced syncytia of cells detaching from the monolayer, which were indistinguishable from those of standard ATue51908, at 56 h postinfection at an MOI of 0.01. (B) In MDBK cells, both full-length recombinant viruses rBRSV and rH/BRSV and standard ATue51908 virus produced similar foci of enlarged cells at 5 days postinfection, whereas the NS2 deletion mutants produced only small foci of degenerating cells.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this work, we describe the cDNA cloning of the entire BRSV genome and the recovery of recombinant BRSV from cDNA constructs.To our knowledge, this is the second species of the genus Pneumovirusfor which the entire genome sequence has been determined and whichhas been made amenable to genetic manipulation. The viruses wehave recovered are derived from a parental virus obtained after12 passages in MDBK cells of BRSV strain A51908, obtained fromthe ATCC. Compared to the published sequences of strain A51908,a marked divergence was observed. The most striking deviationsare located in the SH and G genes, which displayed 86 and 88%amino acid identity, respectively. The parental virus was thereforedesignated ATue51908 (GenBank accession no. AF092942).

The approach used to rescue cDNA derived from ATue51908 into infectious BRSV follows the principles shown to be successfulfor recovery first of recombinant rabies virus (40) and thenof a variety of negative-strand RNA viruses from the rhabdovirus,paramyxovirus, and bunyavirus families (8). It involves simultaneousexpression of viral antigenome RNA and of RNP proteins in orderto promote "illegitimate" encapsidation of the RNA in such a waythat the novel RNP structure may serve as a template for the viralRNA polymerase. The expression systems most widely used rely oninfection of cells with recombinant vaccinia viruses (vTF7-3 orMVA) (2-4, 10, 13, 17, 18, 23, 45) providing T7 RNApolymerase, which is needed for expression of proteins and RNAsfrom transfected plasmids. This, however, requires coping withvaccinia virus-induced CPEs which limit the window for recovery,vaccinia virus-induced recombination of transfected plasmid DNA(13, 18), and separation of different viruses by biophysical(40), biochemical (45), or biological (13) means. We describehere the establishment of a BHK-derived cell line stably expressingT7 RNA polymerase, as first reported for measles virus (32),obviating the use of vaccinia helper virus. Especially for recoveryof BRSV, the availability of a vaccinia virus-free system wasregarded as crucial, since BRSV replicates very slowly and tolow titers in cell culture and is highly cell associated, likevaccinia virus, and since virions are pleomorphic in size andshape, with some particles comparable in size to vaccinia virus.Moreover, a general advantage of the T7 polymerase-expressingcell line in combination with IRES-containing support plasmids(11) was confirmed in the rabies virus recovery system. Comparedto the vaccinia virus-driven expression system, the recovery rateswere increased at least 10-fold (12a).

In contrast to other paramyxoviruses or rhabdoviruses, where N, P, and L proteins are sufficient to support encapsidationof antigenome RNA and to initiate an infectious cycle, recoveryof the pneumovirus HRSV has been shown to require the additionalexpression of the M2 gene (ORF 1), which encodes a transcriptionelongation factor (5, 16). We therefore included a BRSV M2-expressingplasmid in the transfection experiments. Both viruses correspondingto ATue51908, chimeric viruses possessing the leader region ofHRSV, and considerably attenuated NS2-deletion mutants could beisolated from every transfected cell culture dish. The recoveryrate thus exceeds by far 1 in 10⁶ transfectedcells.

The successful recovery of recombinant BRSV indistinguishable in phenotype from the parental virus ATue51908 confirmed theauthenticity and the functionality of the determined nucleotidesequences. A particular focus was laid on the functional characterizationof BRSV sequences previously not available, namely, the gene endsand the L gene. The deduced BRSV L and HRSV L proteins showedamino acid identity of 84% and a similarity of 89%. The aminoacid differences were distributed over the entire protein, indicatingrather identical functions of the two proteins. This finding,and the high degree of similarity of the HRSV and BRSV genomeends, prompted us to see whether the BRSV polymerase would beable to recognize HRSV promoterstructures.

The 3' end of the pneumovirus genome (the genome promoter) contains cis-acting signals directing both transcription of subgenomic,free mRNAs and synthesis of full-length RNPs, as well as sequencesspecifying an encapsidation signal. In the case of HRSV minigenomes,the promoter function was highly sensitive to insertion of nucleotidesinto the terminal 10 residues and into the stretch of residues21 to 25 (6, 7). Interestingly, the eight nucleotide differencesof the BRSV leader region are all located outside of these functionallycritical regions. To determine whether the published HRSV sequencecan substitute for the BRSV genome promoter, chimeras which containthe heterologous HRSV leader region were designed. The chimericviruses could be rescued with the same efficiency as rBRSV andreplicated with the same speed to the same titers and producedthe same type of CPE. The same applied to the chimeric and authenticNS2 deletion mutants (see below). Therefore, the heterologousHRSV leader region is faithfully recognized by the BRSV polymeraseand provides functionally identical signals for RNA transcriptionand replication and for encapsidation of RNAs. The observed nucleotidedifferences apparently do not specify genetic information thatmay account for species specificity, further confirming the closerelationship of BRSV andHRSV.

Members of the genus Pneumovirus show particular features that distinguish them from other paramyxovirus genera, such as thelack of P gene RNA editing. HRSV does not appear to obey the "ruleof six" (35), as do most paramyxoviruses which are able to edittheir P gene RNAs (21). Apparently, this is also true for BRSV.Neither the parental virus ATue51908 nor any of the recombinantshave a genome consisting of multiples of 6 nt. The recombinantBRSV genome lacks five residues compared to the ATue51908 genomebut replicated with the same efficiency. This applies also tothe chimeric H/BRSV, which lacks six residues due to the shorterHRSV leader region. This 1-nt difference was also maintained inthe NS2 deletion mutants BRSV $Delta$ NS2 and H/BRSV $Delta$ NS2. Again, theywere found to replicate at identicalrates.

Another peculiarity of pneumoviruses is the high number of encoded genes, some of which do not have counterparts in otherparamyxoviruses, such as SH, M2, and the nonstructural genes NS1and NS2. It was recently shown that G and SH of HRSV are not essentialfor viral replication in vitro but may enhance membrane fusion(19). A role for the M2 protein as a transcription elongationfactor has also been established (5, 16), but the functionof the two nonstructural proteins NS1 and NS2 has remained ratherobscure. In an artificial minigenome assay, HRSV NS1 and, to alesser degree, NS2, showed inhibitory effects on transcriptionand replication (1). Only revertants of HRSV NS2 knockout viruses,in which tandem stop codons were introduced in such a way thatthe NS2 protein would not be expressed, could be isolated fromplaques observed in transfection experiments (42), indicatingan important function of HRSV NS2 in the virus life cycle. Strikingly,in the avian pneumovirus TRTV, both nonstructural genes are absent,emphasizing the question of whether they represent essential genesin mammalian pneumoviruses such asBRSV.

To address possible functions of NS2 in the virus life cycle, we assembled a BRSV cDNA copy lacking the entire NS2 gene. Thesuccessful recovery of a virus autonomously propagating in BSRcells demonstrated that the NS2 gene is not essential for replicationof BRSV in vitro. The pattern and the relative amounts of mRNAsand full-length virus RNA produced in infected cells were notmarkedly changed, except for the lack of an NS2 transcript. Interestingly,the effect of the NS2 deficiency appeared to be more pronouncedin the bovine MDBK cell line than in BSR cells. Syncytia causedby the NS2-deficient mutants in BSR T7/5 cell monolayers werephenotypically indistinguishable from those caused by standardATue51908. In contrast, BRSV $Delta$ NS2-infected MDBK cells were notenlarged, unlike ATue51908-infected cells. Moreover, maximum titerswere reached in MDBK cells infected with NS2 deletion mutantsby 15 days after infection, compared to 8 days after infectionwith standard ATue51908. In BSR T7/5 cells, maximal final infectioustiters were reached by 5 days after infection, which is comparableto nondeficient viruses. In both cell lines, however, the maximumvirus yield of the NS2 deletion mutants was reduced by a factorof 10 (10⁵ and 10⁴ in BSR T7/5 cells for rBRSV and rBRSV $Delta$ NS2, respectively, and10⁶ and 10⁵ in MDBK cells, respectively). As the cDNA constructs used forrecovery of nondeficient rBRSV were made by completion of theNS2 deletion cDNA, the observed slower growth and the reducedvirus titers are due to the lack of NS2 rather than to putativedifferences in other parts of the genome. Thus, although not essential,NS2 is an accessory factor able to substantially support virusgrowth, by a thus far unknown mechanism. Further experiments usingmodified virus mutants are now feasible and should help to revealthe mechanisms of NS2 involved in facilitating virus growth indifferent celltypes.

The successful recovery of the first BRSV strain from which an entire gene has been deleted is important not only for studyingthe molecular biology and genetics of the virus but also becauseit provides a severely attenuated virus with an unequivocal serologicalmarker. Due to their 3'-proximal locations, NS1 and NS2 are expressedat high levels and induce antibodies in infected calves (44).Further manipulation of NS2-deficient viruses may lead to thedevelopment of attenuated marker vaccines, easily distinguishablefrom wild-type virus. For the prevention of respiratory diseases,live vaccines appear to be best suited due to their ability toconfer local immunity in addition to humoral immune response.It will also be of interest to determine whether foreign epitopesor proteins can be incorporated into the virion in order to designvaccines for other respiratory pathogens or vectors for transientgenetherapy.

	ACKNOWLEDGMENTS

We thank Veronika Schlatt and Karin Kegreiss for perfect technicalassistance.

This work was supported by Intervet International B.V.

	FOOTNOTES

^* Corresponding author. Mailing address: Federal Research Center for Virus Diseases of Animals, Paul-Ehrlich-Str. 28, D-72076Tübingen, Germany. Phone: 49 7071 967205. Fax: 49 7071 967303.E-mail: conzelmann{at}tue.bfav.de.

Present address: Department of Molecular and Cellular Virology, Federal Research Center for Virus Diseases of Animals, D-17498Insel Riems,Germany.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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