Three of the Four Nucleocapsid Proteins of Marburg Virus, NP, VP35, and L, Are Sufficient To Mediate Replication and Transcription of Marburg Virus-Specific Monocistronic Minigenomes

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Journal of Virology, November 1998, p. 8756-8764, Vol. 72, No. 11
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Three of the Four Nucleocapsid Proteins of Marburg Virus, NP, VP35, and L, Are Sufficient To Mediate Replication and Transcription of Marburg Virus-Specific Monocistronic Minigenomes

Elke Mühlberger,^* Beate Lötfering, Hans-Dieter Klenk, and Stephan Becker^*

Institut für Virologie, Philipps-Universität Marburg, 35037 Marburg, Germany

Received 8 June 1998/Accepted 6 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

This paper describes the first reconstituted replication system established for a member of the Filoviridae, Marburg virus(MBGV). MBGV minigenomes containing the leader and trailer regionsof the MBGV genome and the chloramphenicol acetyltransferase (CAT)gene were constructed. In MBGV-infected cells, these minigenomeswere replicated and encapsidated and could be passaged. Unlikemost other members of the order Mononegavirales, filoviruses possessfour proteins presumed to be components of the nucleocapsid (NP,VP35, VP30, and L). To determine the protein requirements forreplication and transcription, a reverse genetic system was establishedfor MBGV based on the vaccinia virus T7 expression system. Northernblot analysis of viral RNA revealed that three nucleocapsid proteins(NP, VP35, and L) were essential and sufficient for transcriptionas well as replication and encapsidation. These data indicatethat VP35, rather than VP30, is the functional homologue of rhabdo-and paramyxovirus P proteins. The reconstituted replication systemwas profoundly affected by the NP-to-VP35 expression ratio. Toinvestigate whether CAT gene expression was achieved entirelyby mRNA or in part by full-length plus-strand minigenomes, a copy-backminireplicon containing the CAT gene but lacking MBGV-specifictranscriptional start sites was employed in the artificial replicationsystem. This construct was replicated without accompanying CATactivity. It was concluded that the CAT activity reflected MBGV-specifictranscription and not replication.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Marburg virus (MBGV) is the prototype member of the family Filoviridae, which belongs to the order Mononegavirales. MBGV causesa severe hemorrhagic disease in monkeys and humans that resultsin high fatality rates. The genomic RNA of MBGV is 19,108 nucleotides(nt) in length (EMBL nucleotide sequence database accession no.Z12132) (5) and is transcribed into monocistronic mRNA speciesencoding seven structural proteins (17, 27). These are a singlesurface protein (GP) inserted in the viral membrane (2, 37),two putative matrix proteins (VP40 and VP24), and the nucleocapsidproteins. In contrast to most rhabdo- and paramyxoviruses, whichare known to possess three nucleocapsid proteins, filovirusescontain one additional protein that is associated with the corecomplex (1, 15). The four nucleocapsid proteins of MBGV arethe nucleoprotein (NP) (3, 33), the L protein (28), andthe viral proteins VP35 and VP30. NP and L are thought to be filovirus-specifichomologues of the nucleoprotein and the polymerase subunit L ofother nonsegmented negative-stranded (NNS) RNA viruses. As thesecond protein encoded in the genome, VP35 is presumed to be theP equivalent of filoviruses. However, VP35 is only weakly phosphorylated(unpublished data) and therefore differs from all P proteins ofother NNS RNA viruses.

In contrast to VP35, the fourth nucleocapsid protein of filoviruses (VP30), encoded by the fifth gene, is highly phosphorylated(reference 15 and unpublished data). The only NNS RNA virusesalso known to possess an additional nucleocapsid protein (M2)are pneumoviruses (18), and the gene coding for M2 is locatedadjacent to the L gene. Recently, Collins and coworkers (8)determined that the M2 protein (also called the 22K protein) ofrespiratory syncytial virus (RSV) is essential for proper elongationof viral mRNAs in a reconstituted, cDNA-expressed RSV minigenomesystem. Furthermore, M2 was found to act as an antiterminatorduring viral transcription (22).

To date, little is known about the function of the different nucleocapsid proteins of MBGV. To obtain more information onthe MBGV replicative cycle and the proteins which are involvedin this process, an artificial replication system based on thevaccinia virus T7 expression system has been established. Suchsystems have been developed previously for various other NNS RNAviruses (9). Briefly, cDNAs of naturally occurring RNA minigenomes(6, 29, 30) or cDNAs of synthetic minigenomes containingleader and trailer regions of the respective viral genome andusually a reporter gene (chloramphenicol acetyltransferase [CAT],luciferase, or viral genes) are inserted in a transcription vectorunder the control of the T7 RNA polymerase promoter (10, 14,21, 24, 32, 35, 38). Cells expressing the T7 RNA polymeraseand the viral proteins essential for replication and transcriptionare transfected with the artificial minigenomic DNA which willbe transcribed by the T7 RNA polymerase. If the minigenome isaccepted as a template by the recombinant viral proteins, virus-specifictranscription and replication will take place, thus mimickingthe authentic viral replication complex. These artificial replicationsystems are helpful tools for the analysis of cis- and trans-actingelements influencing RNA synthesis.

The present study describes the first reverse genetic system for filoviruses. The essential protein components of this systemand the conditions under which transcription and replication takeplace have been determined.

(The contribution of Beate Lötfering was done in partial fulfillment of the requirements for the degree Dr. rer. physiol.from the Department of Medicine of Philipps-Universität Marburg.)

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Viruses and cell lines. The Musoke strain of MBGV, isolated in 1980 in Kenya (34), was grown in E6 cells, a Vero cell line clone (ATCC CRL 1586),as described by Mühlberger et al. (28). For T7 RNA polymeraseexpression, the recombinant vaccinia virus MVA-T7, which was grownin chicken embryo fibroblasts, was used (36).

Molecular cloning. (i) Cloning of nucleocapsid protein genes. cDNAs containing the open reading frame (ORF) of NP, VP35, VP30, and L were cloned into the T7 expression vector pTM1 (kindlyprovided by Bernhard Moss, National Institutes of Health). TheORF and parts of the nontranslated regions of all genes were amplifiedby reverse transcription-PCR (RT-PCR) with specific primers containingappropriate restriction sites. The amplified products were subsequentlyinserted into the EcoRI (for NP) or BamHI (for VP35 and VP30)site of pTM1. The NP construct spans nt 98 to 2377 of the MBGVgenome, VP35 spans nt 2939 to 4337, and VP30 spans nt 8863 to9982; the resulting plasmids were designated pT/NP, pT/VP35, andpT/VP30, respectively. Cloning of the L gene involved synthesisof three PCR fragments. The first (nt 11473 to 13784) was flankedby a SacI-NotI site at its 5' end (mRNA sense) and a BamHI siteat its 3' end and was cloned into the SacI-BamHI sites of thevector pGEM3Zf(+). This clone was designated pGEM/L1.1. The secondfragment (nt 13334 to 15587) was inserted into pGEM/L1.1 by usingthe L-specific restriction sites ClaI and BamHI. The resultingclone, spanning the first 4,408 nt of the L gene, was designatedpGEM/L1. The third fragment (nt 15853 to 18898), amplified tocontain an SphI-NotI site, was inserted into the BamHI and SphIsites of clone pGEM/L1. The resulting clone, pGEM/L, containedthe complete ORF of the L gene. For cloning of L into the vectorpTM1, a NotI linker (Boehringer Mannheim) was ligated into theBamHI site of pTM1 and the L ORF was inserted as a NotI fragment;the resulting clone was designated pT/L.

(ii) Construction of artificial MBGV minigenomes. The first 106 nt of the 3' end of the MBGV genome (leader) were amplified by RT-PCR. For cDNA synthesis, 50 to 100 ng of viralRNA (vRNA) was incubated with a primer complementary to nt 2 to32 of the vRNA (3' end) and containing NcoI and SphI restrictionsites. RT was performed for 40 min at 42°C. The second primerfor PCR was homologous to nt 78 to 106 of the vRNA and containedNotI and BamHI restriction sites. The final concentration of bothprimers was 0.3 µM. PCR conditions were as follows: 35 cyclesof 1 min at 94°C, 1 min at 64°C, and 2 min at 72°C. A 439-nt fragmentof the 5' end (trailer) was generated the same way under the sameconditions. The primer for cDNA synthesis, flanked by a NotI site,was complementary to nt 18670 to 18698 of the vRNA; the secondprimer for PCR was homologous to the last 32 nt of the 5' endand contained NcoI and EcoRI restriction sites. The leader wasdigested with SphI and BamHI and cloned into the vector pGEM3Zf(+).The trailer was digested with NotI and EcoRI and, afterward, wascloned into the pGEM-leader construct. Thus, the 3' and 5' ends(leader-trailer) were joined by a NotI site. The leader-trailerDNA was excised with NcoI, and the overlapping 5' ends (5'-CATG)were partially filled with dCTP, using the Klenow fragment ofDNA polymerase (Boehringer Mannheim; 20 min at 22°C). Thereafter,the remaining overlapping 5' ends were removed by nuclease S1(Boehringer Mannheim) treatment (final concentration, 66 mU/µl;5 min at 37°C), and the fragment was inserted between the StuIand SmaI sites of the transcription vector 2,0 (kindly providedby Andrew Ball, University of Alabama Medical School) (30).As a reporter gene, 668 nt of the CAT gene, flanked by NotI sites,was inserted between the leader and trailer sequences.

For generating negative-strand RNA, the 5' end of the MBGV minigenome was positioned adjacent to the T7 RNA polymerase promoterand the 3' end was followed by the hepatitis delta virus ribozymesequence (Fig. 1A). To obtain MBGV-specific 3' and 5' ends, invitro mutagenesis (Transformer site-directed mutagenesis kit;Clontech) or PCR mutagenesis followed by restriction fragmentreplacement was performed. In vitro transcription of the resultingDNA led to an RNA species with the following extreme genome ends:3'-UC and GG-5'. The NotI site upstream of the CAT gene of thenegative-strand construct was mutated to an NdeI site. Two vacciniavirus-specific transcription terminator regions (21) were insertedinto the plasmid, the first (5'-T₅AT) between the MBGV leaderand the start region of the CAT gene, using the NdeI restrictionsite, and the second (T₈) between the ribozyme sequence and theT7 RNA polymerase terminator. The resulting plasmid was designated215 (Fig. 1A). Since the inserted vaccinia virus transcriptionterminator regions were found to be insufficient to prevent nonspecificCAT activity (see Results), double terminator motifs (5'-NdeI-T₅ATCGCAT₅CT-NdeI),generated with annealed primers, were inserted into the NdeI site.Due to there being a molar excess of the annealed primers duringligation, the terminator motifs were inserted four times in theplus-strand orientation and once in the minus-strand orientation;the resulting plasmid was designated 215_term. For production ofpositive-strand RNA, the fragments were cloned in the reversedirection (plasmid 2.1-CAT) (Fig. 1B). In vitro transcriptionresulted in a plus-strand RNA with the following genome ends:3'-CC and GG-5'.

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FIG. 1. Construction of artificial defective RNAs of MBGV. The minigenomes were inserted in transcription vector 2,0 (gray) between the T7 RNA polymerase promoter and the hepatitis delta virus ribozyme (hatched). For in vitro transcription, plasmids were linearized by using the SalI restriction site (right side). (A) Diagram of negative-sense minigenomic cDNA 215, consisting of 439 nt of the 5' trailer (white) adjacent to the T7 RNA polymerase promoter, 668 nt of the CAT gene in a negative-sense orientation (black), and 106 nt of the 3' leader (white) adjacent to the ribozyme. Above the scheme are indicated the boundary between the T7 RNA polymerase promoter sequence (underlined) and the 5' end of the minigenome (negative-sense orientation) (left side) and the boundary between the ribozyme sequence (underlined) and the 3' end of the minigenome (right side). The CAT gene is flanked by NotI and NdeI restriction sites. (B) Diagram of positive-sense minigenomic cDNA 2.1-CAT, consisting of 106 nt of the 3' leader (white) adjacent to the T7 RNA polymerase promoter, the CAT gene in a positive-sense orientation (black), and 439 nt of the 5' trailer adjacent to the ribozyme sequence (white). The boundaries between the T7 RNA polymerase promoter and the ribozyme sequence (underlined), respectively, and the MBGV-specific sequences are indicated. MBGV-specific sequences are shown in the plus-strand orientation. The CAT gene is flanked by NotI restriction sites. (C) Diagram of the cDNA coding for the copy-back-type negative-stranded minigenome cb-CAT. The minigenome consists of 439 nt of the 5' trailer (white) adjacent to the T7 RNA polymerase promoter, the CAT gene in a negative-sense orientation (black), and, adjacent to the ribozyme sequence, 105 nt complementary to the last 105 nt of the trailer (designated as c-trailer; white), which serves as the leader region. The boundaries between the T7 RNA polymerase promoter and the ribozyme sequence (underlined), respectively, and the MBGV-specific sequences are indicated. MBGV-specific sequences are shown in the negative-sense orientation. The CAT gene is flanked by NotI and NdeI restriction sites. TC start, transcription start site of the NP gene, spanning nt 49 to 60 of the leader region; TC stop, transcription stop site of the L gene, spanning nt 353 to 363 of the trailer region (27). Transcription start and stop sites are indicated only for negative-stranded minigenomes. The cleavage site of the ribozyme is symbolized by a pair of scissors.

Plasmid 215 was used for construction of a copy-back minireplicon (Fig. 1C). Amplification of the last 105 nt of the 5' endof MBGV was performed by RT-PCR with MBGV genomic RNA as a template,a forward primer complementary to nt 19004 to 19036 and containingan NdeI site, and a reverse primer homologous to nt 19087 to 19108of the MBGV genome, which comprises the adjacent 38 nt of theribozyme sequence, including an RsrII restriction site. The 3'leader was removed by digestion of plasmid 215 with NdeI and RsrIIand replaced by the PCR fragment. To provide the authentic NP-specifictranslational start region, the AUG start codon of NP, including7 nt upstream and 5 nt downstream, was inserted in frame withthe CAT gene. In vitro transcription of the constructed copy-backplasmid (cb-CAT [Fig. 1C]) resulted in a negative-stranded RNAwhose first and last 105 nt were complementary.

In vitro transcription. Transcription of minigenome RNA was performed with an AmpliScribe T7 kit (Epicentre Technologies). One microgram of SalI-digestedpurified minigenome DNA was in vitro transcribed in accordancewith the supplier's protocol. After DNase I digestion (0.5 µg/µl),the RNA was purified by using an RNeasy kit (Qiagen) and elutedin 65 µl of H₂O containing 1 U of RNase inhibitor per µl. ForRNA transfection (see below), usually 1 to 10 µl of purified RNAwas used.

RNA transfection of MBGV-infected cells and passaging of CAT activity. Subconfluent E6 cells (approximately 10⁶) were infected with MBGV strain Musoke at a multiplicity of infection (MOI) of 1 PFUper cell. At 1 h postinfection (p.i.), the cells were washed oncewith Dulbecco's modified Eagle medium (DMEM) and transfected with5 to 10 µl of the recombinant RNA, using the transfection reagentDOTAP (Boehringer Mannheim), in a final volume of 2 ml of DMEMas described below. Twenty-four hours later, the medium was replacedby DMEM supplemented with 2% fetal calf serum, and 3 days later,the cells were assayed for CAT activity.

Supernatants of MBGV-infected and -transfected cells were clarified at 5 days p.i. and serially passaged to fresh E6 cells.The cells were harvested and processed for CAT assay and Northernblot analysis.

Combined DNA-RNA transfection of MVA-T7-infected cells. HeLa cells (10⁶ per 7-cm² well) were infected with MVA-T7 at an MOI of 5 PFU per cell. At 1 h p.i., the cells were transfectedwith various amounts of plasmids encoding the nucleocapsid proteinsof MBGV, as indicated in the text as well as in the figures, usingthe Lipofectin (Gibco BRL) transfection technique. At 3.5 h aftertransfection, the cells were washed three times with DMEM withoutfetal calf serum. After the last washing step, the cells wereallowed to stand at 37°C for 15 min. During this time the RNAtransfection reaction mixture was prepared by mixing 80 µl of25 mM HEPES, pH 7.5, with 20 µl of DOTAP. In a separate tube,1 to 10 µl of the in vitro-transcribed minigenome RNA was mixedwith 25 mM HEPES, pH 7.5, to a final volume of 50 µl. The twosolutions were combined, carefully mixed, and incubated for 10min on ice. Two milliliters of DMEM was added, and the RNA transfectionmixture was transferred to the DNA-transfected cells. The plateswere further incubated for 48 to 72 h at 33°C.

CAT assay. CAT activity was determined by using 50 nCi of [¹⁴C]chloramphenicol (Amersham Buchler)/sample in a standard assay (20). ForCAT assays performed with MBGV-infected cells, lysates correspondingto 5 × 10⁵ E6 cells were used. For CAT assays performed with vaccinia virus-infectedcells, lysates corresponding to 10⁵ HeLa cells (1/10 of a 7-cm² well) were used. Quantification of radioactivity was done witha Bio-Imaging Analyzer BAS-1000 (Fujifilm), using TINA software(Raytest).

RNA isolation and MCN treatment. (i) MBGV-infected cells. E6 cells (7.5 × 10⁶) were infected with serially passaged MBGV containing artificial defective RNA particles at an MOI of 10¹ PFU per cell. Cells were lysed at 5 days p.i., and total cellularRNA was isolated by using an RNeasy kit (Qiagen) and subjectedto Northern blot analysis.

(ii) Vaccinia virus system. HeLa cells grown in 7-cm² wells were infected with MVA-T7 and transfected with DNA as described above. At 2 days p.i., cellswere washed two times with phosphate-buffered saline, scrapedinto the washing buffer, and pooled (three wells). After centrifugationfor 10 min at 3,000 rpm in a Heraeus Megafuge 1.0 centrifuge at4°C, the pellets were resuspended in 200 µl of micrococcal nuclease(MCN) buffer (10 mM NaCl, 10 mM Tris [pH 7.5], 1.5 mM MgCl₂, 1%Triton X-100, 0.5% sodium deoxycholate, 10 mM CaCl₂, 1 mM phenylmethylsulfonylfluoride) (16), sheared, and sonicated for 1 min. A 50-µl aliquotof each sample was processed directly for RNA isolation, usingan RNeasy kit (Qiagen). In accordance with the protocol of Fearnset al. (16), the remaining 150 µl of each lysate was treatedwith 3 µl of MCN (Boehringer Mannheim; 15 U/µl) for 75 min at30°C. Subsequently, RNA was isolated by using an RNeasy kit.

(iii) Oligo(dT) purification. Total cellular RNA corresponding to three 7-cm² wells of MVA-T7-infected and transfected HeLa cells was isolated at 2 daysp.i. as described above. Polyadenylated RNA was purified fromtotal RNA by using oligo(dT) cellulose (microcrystalline; NewEngland Biolabs). Unbound and eluted bound RNA were ethanol precipitatedand subjected to Northern blot analysis.

Northern blot analysis. RNA samples were separated on 1.5% agarose gels containing 0.44 M formaldehyde and blotted onto positively charged nylon membranes(Boehringer Mannheim) for 90 min with a vacuum blotter (Appligene),using 3 M NaCl-8 mM NaOH as the transfer buffer (7). Then,RNA was fixed for 3 min by UV cross-linking. Hybridization wasperformed as described by Grosfeld et al. (21). Briefly, membraneswere prehybridized for 6 h at 65°C in a solution consisting of6× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate), 0.1%sodium dodecyl sulfate (SDS), 5× Denhardt's solution, and 0.5mg of denatured, fragmented salmon sperm DNA per ml. After additionof 3 µl of digoxigenin-labeled riboprobe (see below), hybridizationwas done overnight at 65°C. Filters were washed for 5 min at roomtemperature in 0.1× SSC-0.1% SDS and then for 2 h at 65°C in thesame washing solution. Chemiluminescent detection of the hybridizedprobe was performed with CDP-Star in accordance with the supplier'smanual (Boehringer Mannheim). For preparation of positive-strandedriboprobes, 1 µg of the positive-sense minigenomic DNA 2.1-CATwas digested with HindIII and transcribed in vitro, using T7 RNApolymerase and the Dig RNA Labeling Kit (Boehringer Mannheim).For preparation of negative-sense riboprobes, 1 µg of pBluescriptII KS vector containing the CAT gene (BS/CAT) was cut with SacIand in vitro transcribed as described above. After purification,RNA probes were eluted in 100 µl of H₂O.

Western blot analysis. HeLa cells (1.4 × 10⁶) were infected with MVA-T7 and transfected with plasmids encoding the nucleocapsid protein genes of MBGVas described above. After incubation at 37°C overnight, the cellswere washed twice with phosphate-buffered saline and then scrapedinto 500 µl of Triton lysis buffer [20 mM 2-(N-morpholino)ethanesulfonicacid (MES), 55 mM Tris-HCl, (pH 7.8), 200 mM NaCl, 10 mM EDTA,1% (vol/vol) Triton X-100, 5% (vol/vol) Trasylol, 1 mM phenylmethylsulfonylfluoride, 10 mM iodoacetamide). Cell lysates were separated bySDS-polyacrylamide gel electrophoresis (10% gel; 10 µl per lane).Western blot analysis was performed as described elsewhere (2).For detection of NP, a monoclonal antibody raised against NP anddiluted 1:10,000 was used. For detection of VP35, a monoclonalantibody raised against VP35 (a gift of Anthony Sanchez, Centersfor Disease Control and Prevention, Atlanta, Ga.) and diluted1:40,000 was used. For detection of VP30, a guinea pig anti-VP30serum diluted 1:15,000 was used (gift of Heinz Feldmann, Instituteof Virology, Marburg, Germany). Secondary antibodies coupled withperoxidase were diluted 1:100,000 and were detected with SuperSignal Ultra reagent (Pierce). Quantitation of chemiluminescencesignals was done with a Bio-Imaging Analyzer BAS-1000 (Fujifilm),using TINA software (Raytest).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Rescue of an artificial minigenome in MBGV-infected cells. A synthetic defective MBGV-specific cDNA containing the 3' and 5' ends of MBGV RNA and lacking all viral genes, which werereplaced by the CAT gene, was constructed (Fig. 1A). By in vitrotranscription of this construct, an artificial minigenome withnegative polarity (designated as 215) was synthesized. Correct3' ends were generated by autolytic cleavage of the hepatitisdelta virus ribozyme (30). To check whether this RNA constructcould serve as a template for the MBGV replication complex, MBGV-infectedE6 cells were transfected with RNA 215. At 3 to 4 days p.i., thecells were lysed and CAT activity was determined (Fig. 2A). Expressionof the CAT gene was completely dependent on MBGV infection; uninfectedcells transfected with the minigenome (Fig. 2A, mock) were negativefor CAT activity. To prove that the artificial minigenome wasreplicated and could be passaged, clarified supernatants of MBGV-infectedcells transfected with the artificial minigenome were used toinfect fresh E6 cells. At 5 days p.i., cells were lysed to measureCAT activity and supernatants were passaged again to fresh cells.After three passages, CAT activity was still detected, withoutsignificant changes in signal strength, indicating that in factthe artificial MBGV RNA could serve as a template for replication,transcription, and encapsidation (Fig. 2A). These results wereconfirmed by Northern blot analysis. RNA isolated from cells ofthe third passage was hybridized with a positive-sense riboprobe.As shown in Fig. 2B, a specific RNA band (lane b) which was similarin size to the cleaved input RNA (lane d, arrow) was detected.Unexpectedly, an increase in CAT activity as a consequence ofa preferential replication of the small minigenome was not detected.

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FIG. 2. Rescue of minigenomic RNA in MBGV-infected cells. (A) Supernatants of MBGV- or mock-infected E6 cells (mock) that were transfected with the negative-sense RNA 215 were serially passaged to fresh E6 cells. At 5 days p.i., the cells were harvested and assayed for CAT activity. The number of passages is designated as P.0 (transfection) to P.3 (third passage). (B) E6 cells were infected with MBGV (lane a) or with serially passaged MBGV (P.3) containing artificial defective RNA particles 215 (lane b) or were not infected (lane c). At 5 days p.i., total cellular RNA was isolated and subjected to Northern blot analysis. As the probe, a digoxigenin-labeled positive-sense riboprobe DIG-2.1-CAT was used. As a control, in vitro-transcribed RNA 215 was separated on the gel (lane d). The arrowhead marks the position of uncleaved RNA 215 containing the ribozyme; the arrow marks the position of cleaved RNA 215 after removal of the ribozyme.

Expression of MBGV nucleocapsid proteins in MVA-T7-infected HeLa cells. A prerequisite for developing an artificial replication and transcription system for MBGV was the expression of recombinantnucleocapsid proteins. Plasmids encoding NP, VP35, and VP30 underthe control of the T7 RNA polymerase promoter were used to transfectMVA-T7-infected HeLa cells, and protein expression was examinedby Western blot analysis. NP, VP35, and VP30 were transientlyexpressed and migrated on SDS-polyacrylamide gels with the samemobility as the authentic MBGV proteins (data not shown). Sinceantibodies recognizing L were not suitable to detect weakly expressedL, its expression was verified only by its function (see below).

CAT gene expression mediated by MBGV proteins. Next, a study designed to determine which of the four nucleocapsid proteins were essential for MBGV transcription and replicationwas done. HeLa cells were infected with MVA-T7 and transfectedwith plasmid-encoded nucleocapsid genes and the plasmid codingfor the minigenomic RNA 215. Unfortunately, DNA transfection ofplasmids coding for MBGV-specific negative-sense minigenomes containingthe CAT gene led to vaccinia virus-driven CAT gene expression.Grosfeld et al. (21), working with RSV-specific minigenomes,determined that insertion of several vaccina virus-specific transcriptiontermination motifs at different positions in the plasmid eliminatedbackground CAT activity. The MBGV-specific plasmid 215 also containstwo vaccinia virus-specific transcription terminators, but thesedid not prevent nonspecific CAT activity (data not shown).

To abolish nonspecific CAT activity, MVA-T7-infected cells were transfected first with plasmid-encoded nucleocapsid genesand then, 3.5 h later, with in vitro-transcribed negative-strandedRNA 215. At 3 days p.i., the cells were harvested and CAT activitywas determined. Since NP is the most abundant protein of the nucleocapsidcomplex (3), the mixture of plasmids first employed for theseexperiments contained 2 µg of pT/NP, 0.5 µg of pT/VP35, 0.5 µgof pT/VP30, and 1 µg of pT/L. Under these conditions, no reportergene expression could be detected (Fig. 3A, lane 6). However,when the amount of pT/NP was decreased to 100 ng, CAT gene expressionwas observed. Omission of NP, VP35, or L totally abrogated CATactivity, whereas omission of VP30 had no influence on CAT geneexpression (Fig. 3A). These data indicate that NP, VP35, and Lare the key components of MBGV-specific reporter gene expression.

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FIG. 3. Reporter gene expression in cells transfected with plasmids encoding MBGV nucleocapsid proteins and transfected with negative-sense MBGV-specific minigenome 215. HeLa cells were infected with MVA-T7, transfected with pT/NP, pT/VP35, pT/L, and/or pT/VP30, and subsequently transfected with RNA 215. At 3 days p.i., cells were lysed, CAT activity was determined and acetylated products were separated by thin-layer chromatography. (A) DNA transfection was performed with 0.1 (lanes 1 to 5) or 2 (lane 6) µg of pT/NP, 0.5 µg of pT/VP35, 1 µg of pT/L, and/or 0.5 µg of pT/VP30 as indicated. (B) Titration of plasmids encoding the different nucleocapsid proteins. Titration experiments were performed with fixed amounts of three of the plasmids encoding nucleocapsid proteins (pT/NP, 0.1 µg; pT/VP35, 0.5 µg; pT/L, 1 µg; pT/VP30, 0.5 µg) and various amounts of one of the plasmids as indicated at the right side of each panel. (C) Titration of pT/VP35 at large amounts of NP input DNA. DNA transfection was performed with 1 µg of pT/NP, 1 µg of pT/L, and various amounts of pT/VP35 as indicated.

Titration experiments performed with a fixed amount of pT/NP (100 ng) and various concentrations of pT/VP35, pT/VP30, andpT/L revealed that the amounts of VP35 and L input DNA were notvery critical (Fig. 3B, VP35 and L). Optimal results were obtainedby using 0.5 to 1 µg of pT/VP35 and 1 µg of pT/L. Addition ofpT/VP30 up to 2 µg of input DNA did not lead to suppression ofCAT activity (Fig. 3B, VP30). The amount of NP input DNA profoundlyaffected CAT gene expression (Fig. 3B, NP). CAT activity was observedonly with small amounts of pT/NP. Above 0.5 µg of NP input DNA,CAT activity was completely abrogated.

The question of whether it was the absolute amount of NP that was critical for the system or rather the ratio between NP andanother nucleocapsid protein arose. To check whether the NP/VP35ratio influences CAT gene expression, the amounts of both inputDNAs were increased in parallel. As shown in Fig. 3C, reportergene expression was observed even at 1 µg of pT/NP if the amountof pT/VP35 was increased to 5 µg, indicating that it is not theabsolute amount of NP that is critical but rather the ratio ofNP to VP35.

The NP/VP35 ratio in the functional artificial replication system reflects the situation in MBGV-infected cells. Since it was shown that the NP/VP35 input DNA ratio had to be 1:5 to mediate MBGV-dependent reporter gene expression, it wasof interest to determine if this ratio led to NP and VP35 proteinconcentrations which reflected the situation in MBGV-infectedcells. MVA-T7-infected HeLa cells were transfected with fixedamounts of pT/VP35 (0.5 µg) and pT/L (1 µg) and various concentrationsof pT/NP (25 ng to 1 µg). Then, DNA-transfected cells were transfectedwith RNA 215. Cells were harvested, and the cell lysates weresplit and subjected to CAT assay and Western blot analysis (Fig.4). With regard to CAT gene expression, the strongest signal wasobtained at a pT/NP-to-pT/VP35 ratio of 1:5 (Fig. 4A, lane 4).When the ratio was shifted to 1:20 or lower (lane 2) or 1:1 orhigher (lanes 5 and 6), reporter gene expression was totally abrogated.To determine the NP/VP35 ratio at the protein level, Western blotanalyses were carried out with the same lysates and in parallelwith lysates of MBGV-infected cells, using NP- and VP35-specificmonoclonal antibodies. As shown in Fig. 4B, NP expression increasedin response to increasing amounts of transfected pT/NP. The increasein signal strength was linear in the range of 25 to 100 ng ofpT/NP and reached a plateau above 100 ng. The ratio of the chemiluminescencesignals of NP and VP35 in MBGV-infected cells was 6:1 (Fig. 4B,lane 1). A similar value (8.5:1) was detected when the ratio ofthe plasmids encoding NP and VP35 was 1:5 (lane 4). Under theseconditions, the replication system was functional. When the ratioof pT/NP to pT/VP35 was raised to 2:1 (lane 6), expression ofVP35 was strongly suppressed, leading to an NP/VP35 protein ratioof 132:1. From these data taken together, it is evident that theNP/VP35 ratio in MBGV-infected cells is in the range of that observedfor the functional artificial replication system.

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FIG. 4. Determination of the NP/VP35 ratio. HeLa cells seated in 7-cm² wells were infected with MVA-T7 and transfected with 0.5 µg of pT/VP35, 1 µg of pT/L, and various amounts of pT/NP as indicated. At 3.5 h after DNA transfection, cells were transfected with RNA 215. After incubation at 37°C overnight, the cells were harvested. Cell lysates were split and subjected to CAT assay and Western blot analysis. (A) CAT assay performed with 50% of each lysate. (B) Western blot analysis. Lysates corresponding to 3 × 10⁴ cells (lanes 2 to 6) and a lysate of MBGV-infected E6 cells (lane 1) were analyzed by Western blotting with monoclonal antibodies directed against NP (dilution, 1:10,000) and VP35 (dilution, 1:40,000). Chemiluminescence signals specific for NP and VP35 expression were quantified (given in relative densitometer units), and the NP/VP35 ratio was determined (table at bottom). For quantification of NP, degradation products were included. The antibody concentration was adjusted so that the chemiluminescence signals received could be quantitatively evaluated. The signal strength ratios therefore do not necessarily reflect the actual protein ratios.

Replication and encapsidation of MBGV minireplicons. To determine whether the minireplicons were transcribed and/or replicated by recombinant expressed proteins, RNA detectionassays were performed. Using the combined DNA-RNA transfectionprotocol, no MBGV-specific RNA was detected (data not shown).Therefore, the transfection protocol was changed. MVA-T7-infectedcells were transfected with plasmids coding for the supportingproteins and the plasmid encoding the positive-sense minireplicon2.1-CAT. At 2 days p.i., the cells were lysed and total cellularRNA was isolated, treated with MCN, and analyzed by Northern hybridizationwith a positive-sense riboprobe. Minigenomic negative-sense RNAwhich was resistant to MCN treatment was detected, indicatingthat the RNA was replicated and encapsidated (Fig. 5A, lane 3).The protected RNA species comigrated with in vitro-transcribedcleaved RNA 215, which was used as marker (lane 1, arrow). Ashas been shown for reporter gene expression, NP, VP35, and L weresufficient for replication. When the amount of NP input DNA wasincreased, replication was totally inhibited (Fig. 5B). Additionof pT/VP30 was not necessary to support replication, thus confirmingthe results of the CAT assays.

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FIG. 5. Replication of MBGV-specific positive-sense minigenome 2.1-CAT. (A) HeLa cells were infected with MVA-T7 and transfected with 0.1 µg of pT/NP, 0.5 µg of pT/VP35, 1 µg of pT/L, and 0.5 µg of plasmid DNA 2.1-CAT (lanes 3 and 5). As a negative control, pT/L was omitted (lanes 2 and 4). At 2 days p.i., the cells were lysed and the lysates were either treated with MCN (+) (lanes 2 and 3) or were not treated ( $-$ ) (lanes 4 and 5). Then, total RNA was isolated and subjected to Northern hybridization, using the positive-sense digoxigenin-labeled riboprobe DIG-2.1-CAT. As a control, in vitro-transcribed negative-sense RNA 215 was used. The arrowhead indicates uncleaved RNA 215 containing ribozyme; the arrow indicates cleaved RNA 215. (B) HeLa cells were infected with MVA-T7 and transfected with various amounts of pT/NP as indicated, along with 0.5 µg of pT/VP35, 1 µg of pT/L, and 0.5 µg of plasmid DNA 2.1-CAT, without (lanes 1 to 4) or with (lanes 5 to 8) 0.5 µg of pT/VP30. At 2 days p.i., cells were lysed and treated with MCN. Total cellular RNA was isolated and subjected to Northern hybridization with the positive-sense digoxigenin-labeled riboprobe DIG-2.1-CAT.

Transcription of MBGV minigenomes. As mentioned above, DNA transfection with plasmids encoding negative-stranded MBGV minigenomes led to vaccinia virus-drivensynthesis of CAT mRNA because the CAT gene was transcribed byvaccinia virus DNA-dependent RNA polymerases. Like MBGV, vacciniavirus also has the capacity for polyadenylation (19), makingit impossible to distinguish mRNA transcribed by vaccinia virusfrom mRNA transcribed by MBGV proteins. For detection of MBGV-specifictranscription, it was necessary to use a minigenomic DNA whichwas not transcribed by vaccinia virus RNA polymerases. Since transfectionwith plasmid 215 (Fig. 1A), containing two vaccinia virus-specifictranscription terminators at different sites, still led to nonspecificCAT activity (see above), additional vaccina virus transcriptionterminator regions were inserted between the MBGV leader sequenceand the CAT gene. After insertion of an array of eight terminatorsin the plus-strand orientation, background CAT gene expressionwas strongly reduced but not totally abolished (data not shown).However, the resulting plasmid (215_term) was used for cotransfectionof MVA-T7-infected HeLa cells with pT/NP, pT/VP35, pT/L, and pT/VP30.At 2 days p.i., cells were harvested and the lysates were splitand either treated with MCN or not treated. After oligo(dT) purification,the RNA was subjected to Northern blot analysis with a negative-sensedigoxigenin-labeled riboprobe. As shown in Fig. 6A, positive-senseRNA of the predicted size was detected in the unbound and undigestedRNA fraction. The appearance of the specific RNA band was exclusivelydependent on the presence of NP, VP35, and L (Fig. 6A, lane 3),whereas background signals were probably due to vaccinia virus-specificRNA synthesis with plasmid 215_term as the template (Fig. 6A, lane4). A small part of the unbound RNA fraction was shown to be nucleaseresistant, as had been implied for replicated and encapsidatedplus-strand RNA (Fig. 6B, lanes 1 to 3). In the presence of largeramounts of VP30, replication of the minigenome seemed to be inhibited(Fig. 6, lanes 1). However, this effect might be due to an overexpressionof VP30 at 500 ng of VP30 input DNA, since smaller amounts ofVP30 (25 ng of input DNA) did not influence the efficiency ofreplication (Fig. 6B, lane 2). Polyadenylated MBGV-specific RNAwas detected only when the samples were not nuclease treated (Fig.6, lanes 5 to 8), indicating that this RNA species was not encapsidated,as had been predicted for mRNA. The two RNA species, replicatedplus-strand RNA and mRNA, were similar in size. Like replication,transcription of the used monocistronic minigenome was dependenton the presence of NP, VP35, and L as supporting proteins (Fig.6A, lane 7). When L was omitted, specific signals could not bedetected (Fig. 6, lanes 4 and 8). Interestingly, VP30 did notinfluence the synthesis of polyadenylated RNA (Fig. 6A, lanes5 and 6).

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FIG. 6. Transcription of MBGV-specific negative-sense minigenome 215_term. HeLa cells were infected with MVA-T7 and transfected with 0.1 µg of pT/NP, 0.5 µg of pT/VP35, either 25 ng of pT/VP30 (lanes 2 and 6) or 500 ng of pT/VP30 (lanes 1 and 5), 2 µg of plasmid DNA 215_term, and 1 µg of pT/L. As a negative control, pT/L was omitted (lanes 4 and 8). At 2 days p.i., the cells were lysed and either treated with MCN (+) or not treated ( $-$ ). Total cellular RNA was isolated and subjected to oligo(dT) purification. Northern blot analysis was performed with the negative-sense digoxigenin-labeled riboprobe DIG-BS/CAT. The blot exposure time was 30 s (A) or 30 min (B). unbound, RNA fraction which did not bind to oligo(dT) cellulose; bound, RNA fraction that bound to oligo(dT) cellulose; 25, 25 ng of pT/VP30; 500, 500 ng of pT/VP30. The arrows indicate the position of the replicated and transcribed RNA.

CAT activity reflects transcription. As mentioned above, NP, VP35, and L were sufficient to support MBGV-specific reporter gene expression. When MVA-T7-infectedcells, which did not express MBGV proteins, were transfected withpositive-sense minigenome RNA, CAT activity was detected, indicatingthat this RNA could serve as a messenger (Fig. 7A, right panel).Since MBGV-specific replication involves plus-strand RNA intermediates,the question of whether the detected CAT activity generated byMBGV proteins was due entirely to mRNA synthesis $---$ i.e., transcription $---$ orpartly to synthesis of plus-strand minigenomes $---$ i.e., replication $---$ arose.To address this question, an artificial copy-back minirepliconin which the leader region of minigenome 215 was replaced by 105nt complementary to the 5' end of MBGV genome was constructed(cb-CAT [Fig. 1C]). In vitro transcription of cb-CAT resultedin a negative-sense RNA lacking MBGV-specific transcriptionalstart signals upstream of the CAT gene. When MBGV-infected cellswere transfected with cb-CAT RNA, the CAT gene was not expressed(Fig. 7A, left panel). Transfection of control RNA 215 led toCAT gene expression. The same result was obtained when MVA-T7-infectedcells expressing MBGV nucleocapsid proteins were transfected withcb-CAT RNA; i.e., CAT gene expression was not observed (data notshown). However, Northern hybridization carried out with RNA isolatedfrom MVA-T7-infected and pT/NP, pT/VP35, pT/L, and cb-CAT DNA-transfectedHeLa cells demonstrated that cb-CAT RNA was replicated (Fig. 7B).Negative-strand as well as positive-strand RNA was detected. BothRNA species were resistant to MCN treatment. Although plus-strandRNA had been synthesized, no CAT activity was observed. This resultsuggested that CAT activity generated by MBGV proteins was dueto transcription and not to replication. To prove that the CATgene of the cb-CAT plasmid could serve as template for transcriptionand translation, a cassette containing the sequences between theribozyme and the T7 RNA polymerase promoter was cloned into thevector pBluescript II KS under the control of the T3 RNA polymerasepromoter. In vitro transcription by T3 RNA polymerase resultedin a positive-sense RNA (BS/cb-CAT) which was used for transfectionof MVA-T7-infected cells (Fig. 7A, right panel). As a control,plus-stranded 2.1-CAT RNA and negative-stranded RNA cb-CAT wereemployed. Since BS/cb-CAT transfection led to CAT gene expression,it was evident that cb-CAT contained a functional CAT gene, thussupporting the hypothesis that reporter gene expression indeedreflects MBGV-specific transcription.

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FIG. 7. CAT gene expression reflects transcription. (A) Determination of CAT gene expression of cells transfected with copy-back RNA cb-CAT. Left panel: uninfected (mock) or MBGV-infected E6 cells were transfected with RNA cb-CAT or RNA 215. At 3 days p.i., cells were lysed and CAT activity was determined. Right panel: HeLa cells were infected with MVA-T7 and transfected with in vitro-transcribed positive-sense RNA 2.1-CAT, negative-sense RNA cb-CAT, or positive-sense RNA BS/cb-CAT. At 24 h p.i., the cells were lysed and assayed for CAT activity. (B) Replication of copy-back minigenome cb-CAT. HeLa cells were infected with MVA-T7 and transfected with 0.1 µg of pT/NP, 0.5 µg of pT/35, 1 µg of pT/L, and 0.5 µg of plasmid DNA cb-CAT (lanes NP/35/L). As a negative control, pT/L was omitted (lanes NP/35). At 2 days p.i., the cells were lysed and treated with MCN. Duplicate Northern blots were prepared from total cellular RNA, with either in vitro-transcribed positive-sense RNA 2.1-CAT (left panel) or in vitro-transcribed negative-sense RNA 215 (right panel) as a control. Both blots were subjected to Northern hybridization, using either the negative-sense digoxigenin-labeled riboprobe DIG-BS/CAT (left panel) or the positive-sense digoxigenin-labeled riboprobe DIG-2.1-CAT (right panel). The positive-stranded antigenome and the negative-stranded genome are marked by arrows.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this article, a reverse genetic system for MBGV is described. It was shown that three of the four MBGV nucleocapsid proteins,NP, VP35, and L, are sufficient to support replication and transcriptionof monocistronic minireplicons. For various rhabdo- and paramyxoviruses,it is also known that N (NP), P, and L are the minimum proteinrequirements for replication (10, 12, 14, 21, 29, 30,32, 38). For most rhabdo- and paramyxoviruses, the same threeproteins are sufficient to support transcription. Pneumoviruses,however, need an additional transcription factor (8). Comparisonof the primary sequences of MBGV proteins to those of other NNSRNA viruses clearly revealed that MBGV NP and L are homologousto the N (NP) and L proteins of paramyxo- and rhabdoviruses (28,33). Since P proteins are not well conserved among NNS RNA viruses,it is not surprising that the amino acid sequence of VP35 wasnot found to be homologous to any P protein sequence. However,VP35 exhibits some typical features of P proteins: it is encodedby the second gene of the viral genome, and it has been shownto be a nucleocapsid protein that interacts with NP and L (1).On the other hand, there is one striking difference between therhabdo- and paramyxovirus P proteins: MBGV VP35 is only very weaklyphosphorylated. Moreover, for Ebola virus, it has been reportedthat only NP and VP30 are phosphorylated (15). Our observationthat VP35 is essential for MBGV replication clearly indicatesthat this protein is indeed the filovirus-specific P analogue.Therefore, it is proposed that VP35 be renamed P.

Titration experiments performed with the supporting plasmids demonstrated that the amount of NP input DNA was very criticalfor the system. When large amounts of NP DNA were used, CAT geneexpression was completely suppressed. Since reporter gene expressionprobably reflected transcription (see below), one could arguethat small amounts of NP might be sufficient for transcriptionalactivity but not for replication. However, the same effect wasfound for MBGV-specific replication as could be shown by Northernblot analysis. This was surprising because, first, NP is the mostabundant nucleocapsid protein and, second, it was shown for otherNNS RNA viruses that large amounts of NP DNA did not abrogatereplication and/or transcription. For vesicular stomatitis virus,it was demonstrated that increasing amounts of N DNA in the rangeof 15 to 25 µg at fixed amounts of NS (10 µg) and L (5 µg) plasmidDNA did not affect replication of defective interfering particleRNA (31). At larger amounts of N DNA (up to 50 µg), replicationwas decreased but not abrogated. Also, titration of the levelsof N, P, and L plasmids of RSV showed that reporter gene expressionwas maximal when the N and P plasmids were present in equal amounts,but increasing amounts of N input DNA did not reduce CAT geneexpression and replication of minigenomes substantially (21).Comparable results have been obtained for Sendai virus (24).Titration of NP DNA was performed in the range of 0.25 to 2 µg(1 µg of L DNA, 0.5 µg of P DNA) without the loss of reportergene expression. Interestingly, as found with MBGV, reporter geneexpression was affected by changing the relative amounts of thesupporting plasmids. In contrast to MBGV, the amount of P DNAwas particularly critical (24). Additional titration experimentsperformed with MBGV NP and VP35 clearly indicated that it wasnot the absolute amount of NP that was critical for the systembut rather the NP/VP35 ratio. The best results were obtained whenthe NP/VP35 plasmid ratio was 1:5. This ratio was observed tobe optimal for transcription as well as replication. Western blotanalysis of cell lysates obtained from MBGV-infected cells revealedan NP/VP35 ratio of 6:1. This value does not reflect absoluteprotein amounts and is due to the chosen antibody dilutions. SimultaneousWestern blot analyses carried out with MVA-T7-infected and NP,VP35, and L plasmid-transfected cells resulted in a similar NP/VP35ratio when the plasmid ratio was 1:5.

For various NNS RNA viruses it has been said that N (NP) tends to self-assemble. In this form the protein is inactive. Interactionwith P stabilizes the soluble form of N (NP), thus maintainingthe replication complex in an active state (4, 11, 23,26). MBGV NP also has a strong tendency to self-aggregate whichis reflected in the formation of large inclusion bodies intracellularlyby recombinant NP (1). It is hypothesized that the interactionbetween NP and VP35 is critical for keeping NP functional. A definedNP/VP35 input DNA ratio might reflect the stoichiometry of theNP-VP35 complex.

An artificial copy-back minireplicon lacking MBGV-specific transcriptional start sites was found to be a useful tool to differentiatebetween replication and transcription. This copy-back minigenomewas shown to be replicated by MBGV proteins but did not lead toCAT gene expression. When defective minireplicons with authentic3' and 5' ends $---$ i.e., with an active transcriptional start site $---$ wereused for the same experiments, replicated RNA and, in parallel,CAT activity were detected. These data clearly indicated thatCAT gene expression was induced by MBGV-specific mRNA synthesisand not by positive-sense minigenomes. Thus, CAT activity reflectedtranscription and not replication. The fact that reporter geneexpression is linked to viral transcription has also been notedby Kuo et al. (25). RSV minigenomes lacking transcriptionalstart or stop signals induced only minimal amounts of CAT activitycompared to that induced by the nonmutated minireplicon. The twomutants, however, were replicated with the same efficiency asthe nonmutated minigenome. For the bunyavirus system it has alsobeen postulated that CAT activity is due to transcription (13).Since MBGV positive-sense input RNA was accepted as a messengerand hence was translated, the question of why replicated plus-strandedRNA was not translated arose. One possible explanation is thatencapsidation of replicated RNA interfered with translation.

For RSV it has been reported that the fourth nucleocapsid protein, M2, is an essential cofactor for viral transcription, actingas an elongation factor (8) and as an antiterminator (22)during viral transcription. While M2 influences the synthesisof mRNA, reporter gene expression is not dependent on the presenceof M2 (21), i.e., on the proper elongation of the mRNA. Filovirusesalso possess an additional nucleocapsid protein (VP30) which istightly linked to the ribonucleoprotein core (1, 15) andwhich is highly phosphorylated. In this paper, we present evidencethat VP30 is not necessary for replication of monocistronic MBGV-specificminigenomes and, in contrast to M2, is not essential for synthesisof full-length transcripts. Since our experiments were performedwith monocistronic minigenomes, it must be elucidated whetherVP30 plays a role during replication and transcription of polycistronicRNA.

	ACKNOWLEDGMENTS

We thank Angelika Lander for expert technical assistance. We are very grateful to R. M. Elliott for critical reading of themanuscript. We thank A. Ball for supplying the transcription vector2,0.

This work was supported by the Deutsche Forschungsgemeinschaft (SFB 286) and the Kempkes Stiftung (21/95). B. Lötfering wasthe recipient of a fellowship from the Graduiertenkolleg Zell-und Tumorbiologie.

	FOOTNOTES

^* Corresponding author. Mailing address for Elke Mühlberger: Institut für Virologie der Philipps-Universität Marburg, Robert-Koch-Str.17, 35037 Marburg, Germany. Phone: 6421-285433. Fax: 6421-285482.E-mail: muehlber{at}mailer.uni-marburg.de. Mailing address for StephanBecker: Institut für Virologie der Philipps-Universität Marburg,Robert-Koch-Stro 17, 35037 Marburg, Germany. Phone: 6421-285433.Fax: 6421-285482. E-mail: becker{at}mailer.uni-marburg.de.

REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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38. Yu, Q., R. W. Hardy, and G. W. Wertz. 1995. Functional cDNA clones of the human respiratory syncytial (RS) virus N, P, and L proteins support replication of RS virus genomic RNA analogs and define minimal trans-acting requirements for RNA replication. J. Virol. 69:2412-2419[Abstract].

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