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Journal of Virology, September 1999, p. 7787-7794, Vol. 73, No. 9
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Institute of Virology and Immunoprophylaxis, CH-3147 Mittelhäusern, Switzerland
Received 3 November 1998/Accepted 9 June 1999
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ABSTRACT |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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To determine the minimal requirements for autonomous RNA replication of classical swine fever virus (CSFV), genomes having in-frame deletions within the genes for structural and flanking nonstructural proteins were constructed, based on an infectious cDNA clone of CSFV Alfort/187. RNA was transcribed in vitro from the respective plasmids and transfected into SK-6 swine kidney cells. The replication competence of the RNA was determined by immunostaining transfected cells for CSFV NS3 protein and by analysis of cell extracts for viral RNA, as well as protein synthesis at different times after transfection. The genes encoding Npro, C, Erns, E1, E2, p7, and NS2 proved to be dispensable for RNA replication, but the efficiency of replication varied strongly between individual constructs. RNA replicons containing the complete NS2-NS3 gene persisted in transfected cells and continued to replicate without causing any obvious morphological or functional damage to the cells, whereas genomes lacking the NS2 gene replicated more efficiently and induced a cytopathic effect. These findings suggest that NS2, although it is not essential for pestivirus RNA replication, has a regulatory function therein. Both cytopathogenic and noncytopathogenic replicons were packaged into virus particles provided in trans by a cotransfected full-length helper virus genome.
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INTRODUCTION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Classical swine fever virus (CSFV) is the causative agent of a highly contagious disease in pigs. Virulent strains cause characteristic disease symptoms such as fever, neurological disorders, hemorrhages, and high mortality rates, whereas infection with avirulent strains remains clinically inapparent but induces a protective immunity. Furthermore, prenatal infection of fetuses can lead to persistently infected animals which shed virus over a long period, as do pigs which exhibit the chronic form of disease (3, 4, 29, 31).
CSFV, bovine viral diarrhea virus (BVDV), and border disease virus form the pestivirus genus within the family Flaviviridae (33). CSFV is a small enveloped virus containing a positive-strand RNA genome of 12.3 kb, which consists of a 5' untranslated region (5'UTR), a large open reading frame (ORF) encoding a single polyprotein, and a 3' untranslated region (3'UTR) (16, 29). The 5'UTR contains an internal ribosomal entry site for cap-independent translation initiation of the viral polyprotein which is co- and posttranslationally processed by host cell and viral proteases (reviewed in reference 16). The cleavage sites of the polyprotein have been determined for BVDV, except for p7-NS2 (5, 16, 23, 26). C, Erns, E1, and E2 represent the structural proteins found in mature virions. As demonstrated for other flaviviruses (2), RNA replication of pestiviruses is thought to occur on cytoplasmatic membranes via the synthesis of a negative-stranded full-length genome (6, 7, 23), while the components of the viral replication complex have not been identified. It has been shown recently that the viral protein NS5B of BVDV has RNA-dependent RNA polymerase activity (37). The NS3 protease is responsible for the cleavage of the viral polyprotein downstream of NS3 and requires NS4A as a cofactor (28, 35). Furthermore, it possesses both helicase and NTPase activity (27, 32), suggesting a role in RNA replication.
According to their behavior in tissue culture pestiviruses can be divided into two biotypes, noncytopathogenic (NCP) and cytopathogenic (CP). The mechanism responsible for the cytopathic effect (CPE) is poorly understood, but the overexpression of NS3 is a common feature of all CP pestiviruses (16). Furthermore, it has been shown that cells infected with CP BVDV undergo apoptosis (10, 36). CP pestiviruses represent mutants which arise from NCP viruses, presumably by RNA recombination during replication (16). Several mutants have been described for BVDV. Most of them contain rearrangements of viral sequences and/or insertions of host cell sequences (reviewed in reference 16). However, some CP BVDV and all CP CSFV isolates described so far are composed of defective interfering (DI) particles and NCP helper virus. CSFV DI genomes, with the identical deletion of 4,764 nucleotides (nt) corresponding to the genes encoding Npro through NS2, have been isolated from different sources (12, 14, 17). A genome with a similar deletion of 4,746 nt has been described recently (12). Furthermore, a defective genome was reported which lacks the 4,263 nt encoding C through NS2 but retains the foreign murine ubiquitin gene which had been used to replace Npro at the 5' terminus of the ORF in the parental genome (30). After transfection into susceptible cells, such defective CSFV genomes, obtained either by extraction from infected cells or by transcription in vitro from the respective cloned cDNA, replicate and are packaged efficiently in the presence of helper virus RNA, thereby causing a CPE (14, 15).
An autonomously replicating defective BVDV genome which lacks the genes encoding C, Erns, E1, E2, p7, and NS2 has been described recently by Behrens et al. (1). It demonstrates that none of these proteins is essential for RNA replication. In the same study it was suggested that the 5' terminal region of the ORF contains a cis signal required for RNA replication, since the Npro gene could neither be deleted completely nor be replaced by a ubiquitin gene. However, the replacement of the Npro gene by ubiquitin in the CSFV Alfort/187 genome yielded infectious virus (30).
In this report a series of in vitro-constructed defective CSFV genomes derived from strain Alfort/187 were analyzed with respect to autonomous RNA replication in SK-6 cells. The question of whether these defective genomes can be packaged in the presence of a helper virus and whether they are cytopathogenic was also addressed.
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MATERIALS AND METHODS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Cells and viruses. The swine kidney cell line SK-6 (11), kindly provided by M. Pensaert (Faculty of Veterinary Medicine, Ghent, Belgium), was propagated in Dulbecco's modified Eagle medium supplemented with 5% horse serum. CP CSFV vA187-1 used as a control was derived from a persistently infected SK-6 cell culture in which DI particles had been spontaneously generated (17).
Plasmid constructs.
Plasmids were amplified in
Escherichia coli XL-1 Blue cells (Stratagene). Restriction
enzymes were purchased from New England Biolabs except for
SrfI (Stratagene). Plasmid DNA was purified with the Wizard
Mini- or Maxiprep kit (Promega). Primers used for reverse transcription
(RT) and PCR are shown in Table 1. Mutant
CSFV genomes shown in Fig. 1 were
constructed on the basis of the full-length cDNA clones pA187-1
(25) and pA187-CAT (20). CSFV-specific
restriction sites are indicated by superscript numbers corresponding to
their positions on the genome of vA187-1 (25).
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(i) pA187-
p7, pA187-3390, and pA187-4263.
The
ExSite PCR-based site-directed mutagenesis kit (Stratagene) and primer
pairs NS2-LMfe and E2-RMfe (p7), NTR-R and NS2-L (3390), and
Npro-R and NS3-L (4263) were used to construct these
deletion mutants. In the following description, CSFV-specific
restriction endonuclease sites are given with their positions
(indicated by superscript numbers) in the viral genome. Since the
cleavage site between p7 and NS2 and, therefore, the exact 5' terminus
of the NS2 gene is not known, the 3' borders of the deletions in the
constructs A187-3390 and -p7 were chosen within the genome region
suggested by Elbers et al. (5) to contain the respective
cleavage site. Two pBluescript-derived subclones of pA187-1 were used
as templates for mutagenesis PCR: pBS-E/K-A187, containing the
EagI82 to KpnI4453
fragment of pA187-1, and pBS-T7G1P (25), containing the
EagI82 to BamHI6437
fragment of pA187-1. Deletions and flanking regions were confirmed by
DNA sequencing. Fragments AflII3396 to
KpnI4453, EagI82 to
KpnI4453, and BspDI778 to
NcoI5533, each carrying the appropriate
deletion, were isolated and used to replace the corresponding fragment
in pA187-1 to obtain pA187-p7, -3390, and -4263, respectively.
(ii) pA187-E2.
The SpeI2429 to
AflIII3000 fragment of pA871-1 was subcloned
into pBluescript to obtain pBS-E2. This plasmid was cleaved with
NheI2444 and EcoNI2906,
treated with Klenow polymerase, and religated. A clone with an in-frame
deletion ranging from nt 2443 to 2907 was identified by DNA sequencing,
and the SpeI2429 to
AflIII3000 fragment of this clone was used to
replace the corresponding fragment in pA187-1 and pA187-CAT to produce
pA187-E2 and pA187-E2-CAT, respectively.
(iii) pA187-Apa and pA187-Acc.
Plasmid pBS-E/K-A187
was digested with ApaI660,3260 or with
AccI445,4407 and religated. From the resulting
plasmids, the respective EagI82 to
KpnI4453 fragment, comprising either a 2,601-nt
or 3,963-nt in-frame deletion, was replaced in pA187-1, to obtain
pA187-Apa and pA187-Acc, respectively. Similarly,
pA187-Apa-CAT and pA187-Acc-CAT were derived from pA187-CAT via
the subclone pBS-E/K-A187-CAT.
(iv) pA187-4764 and pA187-4764Ubi.
Defective CSFV
genomes carrying these deletions were spontaneously generated in SK-6
cells persistently infected either with biologically cloned strain
Alfort/187 (17) or vA187-Ubi (30). To generate
molecular clones of these genomes, viral RNA was extracted from the
respective cell culture medium and subjected to RT-PCR with the primers
CSF-L001 and PR5 as described before (20). The resulting PCR
products of 832 and 1,060 bp, respectively, were digested with
EagI82 and NcoI5533 and
used to replace the corresponding fragment in pA187-1, to obtain
pA187-4764 and pA187-4764Ubi, respectively.
(v) pA187-4764BN.
pA187-4764 was digested with
BspEI5460 and NcoI5533,
treated with Klenow polymerase, and religated. The presence of the
predicted in-frame deletion of 69 nt within the protease domain of NS3
was confirmed by DNA sequencing.
In vitro transcription and electroporation. In vitro transcription from SrfI12298- or NruI11301-linearized plasmids was performed by using the T7 Megascript kit (Ambion) as described before (20, 25, 30). After DNase I digestion, transcripts were purified through MicroSpin S-400 HR columns (Pharmacia) and quantified with a GeneQuant II photometer (Pharmacia). SK-6 cells were washed twice and resuspended in ice-cold phosphate-buffered saline (PBS). A total of 2 × 107 cells in a volume of 0.8 ml were mixed with 15 µg of RNA, transferred to a 0.4-cm cuvette (Bio-Rad), and electroporated immediately by using a Gene Pulser (Bio-Rad) set at 450 V and 500 µF. Alternatively, 0.4 ml of cell suspension at a density of 107 cells/ml was mixed with 5 µg of RNA, transferred into a 0.2-cm cuvette, and electroporated twice at 200 V and 500 µF. After electroporation the cell suspension was kept for 10 min at room temperature, then diluted in Dulbecco's modified Eagle medium containing 5% horse serum, seeded, and harvested for analysis at different times after electroporation.
Cell staining. After electroporation 4 × 105 cells per well were seeded in 24-well plates and heat fixed at the indicated time as described before (17). For the terminal deoxynucleotidyltransferase-mediated dUTP-biotin nick end labelling (TUNEL) assay performed with the in situ cell death detection kit (Boehringer Mannheim) cells were seeded in 96-well plates at a density of 4 × 104 cells per well. Fixation and staining were performed as suggested by the manufacturer. After heat fixation or TUNEL assay the cells were incubated overnight at 4°C with primary antiviral antibody diluted in PBS containing 0.01% Tween 20. Monoclonal antibodies (MAb) C16 (9, 21) and HC/TC 26 (8) were used for the detection of NS3 and envelope protein E2, respectively. Bound primary antibody was labelled with biotinylated anti-mouse antibody (LSAB kit; DAKO) and streptavidin-horseradish peroxidase conjugate (LSAB kit; DAKO) and visualized by adding chromogen solution (17). The cells were examined by fluorescence and bright-field microscopy to identify TUNEL-positive and immunostained cells, respectively.
RNA analysis. Total RNA was extracted from 5 × 106 electroporated cells with Trizol reagent (Gibco). Irrespective of the RNA concentration, one-third of each sample was used for Northern blotting in order to standardize the samples based on the number of electroporated cells. Northern blotting and hybridization were performed as described before (17) with 32P-labelled riboprobes: either JL1, which is complementary to the 3'-terminal 204 nt, for the detection of positive-stranded viral RNA of the CSFV Alfort/187 genome, or GM, corresponding to nt 327 to 582 of the CSFV Alfort/187 genome for the detection of negative-stranded RNA.
RT reactions were performed by using the Expand RT kit (Boehringer Mannheim), primer HR3, and MicroSpin S-400 HR columns for subsequent cDNA purification (17, 20). For PCR either the Expand long-template PCR kit (Boehringer Mannheim) or, for amplification of fragments shorter than 1 kb, Taq DNA polymerase (Promega) was used.Protein analysis. SK-6 cells were lysed in a hypotonic buffer (20 mM MOPS [morpholinepropanesulfonic acid], 10 mM NaCl, 1.5 mM MgCl2, 1% Triton X-100 [pH 6.5]), and the extracts were used either for chloramphenicol acetyltransferase-enzyme-linked immunosorbent assay (CAT-ELISA) (Boehringer Mannheim) or for Western blotting as described before (17, 20). Porcine antipestivirus hyperimmune serum N8T12 (19) and MAb 49DE directed against pestivirus NS3 (kindly provided by E. Peterhans, Institute of Veterinary Virology, University of Bern, Bern, Switzerland) served for the detection of NS3.
Packaging of replicon RNA. After electroporation of defective genomes together with full-length helper A187-CAT RNA, 5 × 106 SK-6 cells were incubated for 48 h before the virus was harvested by freezing and thawing of the cultures. After low-speed centrifugation, 1 ml of undiluted supernatant was used to infect 2 × 106 SK-6 cells seeded the day before and the inoculum was replaced after 1 h. An aliquot of the cell culture medium was collected 48 h after infection for RNA extraction and RT-PCR, which was performed as described before (20).
CPE assay. CPE induced by replicon RNA was monitored on SK-6 cells seeded at a density of 1.5 × 105 (for subsequent infection) or 4 × 105 (after electroporation) per well in 24-well plates. For infection, virus obtained either from the cultures in which the packaging had been performed or from cultures in which the respective packaged replicons had been passaged once or twice was used. Undiluted supernatant obtained after centrifugation of the respective frozen and thawed cultures served as the inoculum, which was replaced with fresh medium 1 h after infection. The cells were examined twice a day by light microscopy for the development of a CPE. After 48 or 72 h the medium was removed, and the cells were fixed and stained by the addition of a crystal violet solution (0.4 mg of crystal violet per ml and 0.37% formaldehyde in PBS) for 1 h to visualize the CPE macroscopically.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Replication competence of defective genomes. The defective genomes shown in Fig. 1 were transcribed in vitro from the respective plasmids, and 15 µg of each RNA was transfected into 2.5 × 107 SK-6 cells. Subsequently, the cells were split in order to perform immunostaining (Fig. 2), to analyze viral RNA (Fig. 3 and 4) and viral protein expression (Fig. 5) at different times after electroporation.
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Apa (Fig. 2C), -4764Ubi (Fig. 2H), or
-4764 (Fig. 2I) RNA scored positive at 16 h after electroporation, but the latter two showed a more intense staining than
A187-Apa. A lower percentage of NS3-positive cells was observed after electroporation of A187-E2 (Fig. 2B), -3390 (Fig. 2D), and
-4263 (Fig. 2G), whereas no stained cells were found after electroporation of either A187-p7 (Fig. 2A), -Acc (Fig. 2E), -4764BN (Fig. 2K), or of 3' truncated A187-Apa RNA (Fig. 2F). The proportion of NS3-expressing cells remained constant between 16 and
44 h after electroporation in the case of A187-E2 (Fig. 2B),
-Apa (Fig. 2C), and -3390 (Fig. 2D). In contrast, both the
proportion of cells positive for NS3 and the total number of cells were
significantly reduced at 44 h after electroporation of
A187-4263 (Fig. 2G), -4764Ubi (Fig. 2H), and -4764 (Fig. 2I)
when compared to 16 h after electroporation. The absence of wild-type CSFV in the electroporated cells was confirmed by
immunostaining for CSFV E2 with the MAb HC/TC 26 (data not shown).
Northern blotting was performed with total RNA extracted from
electroporated SK-6 cells 1, 20, and 48 h after electroporation (Fig. 3A to D). The blots shown in Fig. 3A to C were hybridized with
the negative-stranded RNA probe JL1 complementary to the 3'UTR of CSFV.
As no detectable amounts of positive-stranded RNA were expected to be
synthesized 1 h after transfection, this time point served for
analysis of the stability of the different RNAs. Although equal amounts
of RNA were electroporated the hybridization signals obtained for viral
RNA extracted after 1 h varied considerably for the different
transcripts (Fig. 3A). The low concentration of transcripts found for
cells transfected with A187-E2 and A187-Acc RNA suggests that
these RNAs are rapidly degraded. As expected, no signal was obtained
for the transcript derived from NruI-linearized plasmid,
since it lacked the 3'UTR to which the riboprobe was complementary.
Total RNA extracted 20 h after electroporation (Fig. 3B) contained
increased amounts of positive-stranded viral RNA for A187-4764Ubi
and A187-4764 RNA, and, less pronounced, for A187-Apa RNA. At
48 h after electroporation (Fig. 3C), the signal was further
increased in the case of A187-Apa RNA, whereas it was reduced for
A187-4764 RNA and absent for A187-4764Ubi RNA. The strong decline
in detectable RNA for the latter two constructs was expected due to the
almost complete destruction of the respective cultures by these
cytopathogenic replicons. Negative-stranded viral RNA corresponding in
size to the respective input positive strand was detected at 20 h
after electroporation of A187-Apa, -4764Ubi, and -4764
transcripts, but the amounts were significantly larger for the latter
two RNAs (Fig. 3D). The specificity of the riboprobe used for the
detection of negative-stranded viral RNA was confirmed by hybridization
to in vitro transcripts of pA187-1 of negative and positive polarities
(Fig. 3D). For A187-E2 and A187-4263 RNA a signal for
positive-stranded viral RNA of the predicted size was observed both at
20 and 48 h after electroporation, and for A187-3390 RNA at
48 h but not at 20 h (Fig. 3B and C). However, negative
strands of these viral RNAs could not be detected (Fig. 3D).
Transcripts from SrfI-linearized pA187-p7, -Acc, and
-4764BN and from NruI-linearized pA187-Apa did not
yield detectable amounts of input-sized RNA of either polarity 20 and 48 h after electroporation (Fig. 3B to D).
One-fifth of the total cellular RNA extracted 48 h after
electroporation was digested with RNase-free DNase to remove traces of
plasmid DNA prior to performing CSFV-specific RT-PCR with primers HL3
and HR3. A 241-bp fragment of the NS3 gene present in all deletion
mutants was amplified from all samples except for RNA from
mock-electroporated cells (Fig. 4). The RT-PCR was also positive for
the two RNAs designed not to replicate, namely the 3' truncated A187-Apa RNA transcribed from NruI-linearized plasmid,
and A187-4764BN RNA which has a deletion within the NS3 protease domain.
To confirm the expression and processing of the viral polyprotein by
defective genomes, 5 × 106 electroporated SK-6 cells
were lysed 20 h after electroporation, and the extracts were
subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis
and Western blotting. MAb 49DE9 and porcine hyperimmune serum N8T12
served for the detection of NS3 expressed by RNA replicons (Fig. 5).
Cells electroporated with either A187-4764Ubi or A187-4764 RNA
expressed NS3 which comigrated with the respective protein obtained
from cells infected with CP vA187-1. NS3 protein was also expressed
from A187-4263 RNA, yet in smaller amounts. From the other RNAs
(A187-p7, -E2, -Apa, -3390, -Acc, and -4764BN) no
NS3 or NS2-NS3 expression was detected.
The expression of viral proteins by the replicons A187-E2 and
A187-Apa was further confirmed via a marker gene. The corresponding constructs pA187-E2-CAT, -Apa-CAT, and -Acc-CAT are derived from pA187-CAT (20), a full-length cDNA clone containing the CAT marker gene close to the 5' end of the ORF within the
Npro gene. Immunoperoxidase staining of cells
electroporated with the respective in vitro transcripts revealed
similar proportions of NS3-positive cells as observed with the
corresponding constructs which did not contain the CAT gene (data not
shown). CAT protein was detected by ELISA in hypotonic cell lysates
harvested 20 h after electroporation (Fig.
6A). A time course experiment confirmed that both A187-E2-CAT and A187-Apa-CAT expressed the marker protein (Fig. 6B). In contrast, electroporation of transcripts from
SrfI-linearized pA187-Acc-CAT or pA187-E2 or from
NruI-linearized pA187-Apa-CAT did not yield detectable
amounts of CAT protein (Fig. 6A and B).
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4764 was
sequenced, five point mutations were identified when compared to the
authentic sequence of pA187-1. In contrast, no mutations were found in
the respective fragments of pA187-4764Ubi and pA187-4764iv (Fig.
1), which was constructed in vitro from a subclone of pA187-1 in
analogy to pA187-4263 with primers NS3-L and NTR-R (Table 1). RNA
transcribed from pA187-4764 and pA187-4764iv had
indistinguishable properties in terms of transfection efficiency,
protein expression, and cytopathogenicity (data not shown), indicating
that the five mutations in pA187-4764 did not alter its phenotype.
Packaging of replicons in virus particles.
To show the
packaging of viral RNA, SK-6 cells were coelectroporated with helper
A187-CAT RNA and the respective defective RNAs. At 48 h after
transfection the cell-free supernatants were collected and used to
infect SK-6 cells. The medium of these cultures was collected 48 h
postinfection. The RNA was extracted and used to perform RT-PCR with
the CSFV-specific primers Pest1 and PR5. A 5.8-kb product representing
the A187-CAT helper genome was amplified from all samples except for
those containing either A187-4764Ubi or A187-4764 RNA, which both
had caused an extensive CPE. Shorter PCR products corresponding in
length to the input replicon RNAs were detected for A187-Apa,
-4263, -4764Ubi, and -4764 (Fig. 7A). An additional PCR specific for the
marker gene of the helper virus confirmed the presence of vA187-CAT in
all samples derived from coelectroporations with the respective in
vitro transcript (Fig. 7B).
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Cytopathogenicity of replicons.
Cell morphology and
immunostaining after electroporation suggested that the replicons
A187-4263, -4764Ubi, and -4764 were cytopathogenic (Fig. 2G,
H, and I). To further characterize the cytopathogenic nature of
replicons, SK-6 cells were electroporated with the respective RNAs and
examined 20 h later by TUNEL assay for fragmentation of genomic
DNA as a marker for cell death as well as for the expression of NS3. A
high percentage of the cells scored positive in the TUNEL assay in all
cultures including mock-electroporated cells (Table
2). This was likely due to the
electroporation procedure, which causes extensive damage of the cells.
Thus, the defective genomes were packaged into virions by
coelectroporation of SK-6 cells with helper A187-CAT RNA as described
above. As expected, CPE was observed in cells coelectroporated with
helper RNA and, more dramatically, after passage of the supernatants
for the transcripts A187-4263, -4764Ubi, and -4764 but not for
any of the other defective RNAs or for helper RNA alone (Table 2).
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4263, -4764Ubi, or
-4764 RNA induced CPE as observed by microscopy (Table 2). Foci of
rounded cells typical for CSFV-induced CPE contained a high proportion
of TUNEL-positive cells (Table 2). These cells were also intensively
stained for NS3. However, not all cells positive for NS3 were also
positive in the TUNEL assay. A separate immunostaining with MAb HC/TC26
directed against E2 revealed that 100% of the cells were infected with
helper virus (data not shown).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In order to define the genes required for RNA replication of CSFV,
a series of defective genomes carrying deletions within the 5' half of
the ORF was constructed, based on the infectious full-length clones
pA187-1 and pA187-CAT. The genes encoding Npro through NS2
proved to be dispensable for RNA replication, since A187-4764 RNA
replicated autonomously. As replicon RNA with partially or completely
deleted structural genes is not expected to spread from cell to cell, a
highly efficient transfection procedure was required to detect low
levels of RNA replication. In fact, for the defective genomes
A187-Apa, -4764Ubi, and -4764, more than 50% of the cells
stained positive for NS3 16 h after electroporation (Fig. 2C, H,
and I), and direct evidence for replication was obtained by the
detection of negative-stranded RNA of these genomes (Fig. 3D). In
contrast, no NS3-positive cells were observed after electroporation of
a 3' truncated transcript from pA187-Apa. Lower proportions of cells
staining positive for NS3 were observed for A187-E2, -3390, and
-4263 RNA. We conclude that these mutant genomes are replicons as
well and that negative-stranded RNA could not be detected due to a less
efficient transfection and/or replication of these genomes.
Furthermore, in cells transfected with A187-E2-CAT or
A187-Apa-CAT the marker protein CAT was expressed but not after
transfection of the respective 3' truncated RNAs or A187-Acc-CAT (Fig. 6). This confirms the result obtained with immunostaining for NS3
and shows that translation from input RNA does not yield detectable
amounts of protein. The concentration of CAT for the replicons
A187-E2-CAT and A187-Apa-CAT was only slightly above the
detection limit of the ELISA and about 100-fold lower than for
infection of SK-6 cells with vA187-CAT (19). Nevertheless, this shows that CAT is a useful marker for the detection and
quantification of replication of mutant CSFV genomes.
The RNAs A187-p7, -Acc, and -4764BN did not replicate at
detectable levels (Fig. 2). This was expected for the latter construct,
since the serine protease domain is essential for replication (13,
35). In contrast, the constructs A187-p7 and A187-Acc contain all genes required for replication (Fig. 1). We speculate that
these RNAs might have an altered secondary structure which affects
their ability to serve as a template for RNA replication or
translation, since sequencing the template plasmids revealed no
mutations which could account for a failure to replicate.
Alternatively, correct processing of the viral polyprotein might be
affected by the deletions in the E2-p7-NS2 region, yielding
nonfunctional proteins. Although the amount of input RNA was
standardized, the transfection efficiency as reflected by the
proportion of NS3-positive cells 16 h after transfection varied
from below 1% to nearly 100%, depending on the construct (Fig. 2).
Furthermore, the amount of RNA detected in cells 1 h after
transfection varied strongly, indicating that the stability of the
respective transcripts varies. We exclude the possibility that the RNA
detected at this time by Northern blot analysis represents newly
synthesized RNA. Even after infection of SK-6 cells with wild-type CSFV
at a multiplicity of infection of 10 and by using the same detection
procedure, we have never observed viral RNA earlier than 6 h after
infection (18). Differences in RNA stability might also be
responsible for the strong variation in the transfection efficiency
between individual constructs (Fig. 2). In addition, it has to be
considered that in vitro transcripts of different constructs do not
necessarily yield equal proportions of RNA molecules with a correct,
replication-competent secondary structure. Thus, we conclude that the
number of input RNA molecules required to start replication in a single
cell varies according to the nature of the particular construct.
We cannot exclude that in the case of constructs with low transfection
efficiency, such as A187-3390, the few cells which stain positive
for NS3 (Fig. 2D) contain RNA with an altered sequence compared to its
parental template plasmid. In this case, the replicating RNA might have
acquired mutations either during in vitro transcription by T7 RNA
polymerase or during initial low-level replication in cells. To obtain
sufficient material for sequencing and identification of such
mutations, RT-PCR amplification of these genomes would be required.
However, virus-specific RT-PCR yielded strong signals 48 h after
electroporation (Fig. 4), even for genomes unable to replicate such as
A187-4764BN or A187-Apa RNA lacking its 3'UTR. This
demonstrates that input RNA remains detectable over a long time and,
therefore, that sequencing of RT-PCR products would be biased.
Interestingly, two types of RNA replicons were found with respect to
their replication kinetics and their effect on host cells. The
defective genomes A187-E2, -Apa, and -3390 represent the noncytopathogenic replicon type, whereas A187-4263, -4764Ubi, and
-4764 are cytopathogenic replicons. NCP replicons encode NS2-NS3,
replicate at low levels, and persist in transfected cells for at least
10 cell passages (data not shown). NS3 expressed by NCP A187-Apa was
detectable by immunostaining in the majority of the electroporated
cells and barely on Western blots, indicating that the expression level
is significantly lower than that for CP replicons or virus infection
(Fig. 5). On the other hand, CP replicons which do not contain the NS2
gene replicate very efficiently and express large amounts of NS3 (Fig.
2 and 5), the latter being the common feature of CP pestiviruses
(16). No functions of pestivirus NS2 have been identified so
far (16), but in the closely related hepatitis C virus it
was suggested to be involved in the processing of NS2-NS3
(34). Our findings indicate that CSFV NS2 has a regulatory
function in RNA replication; nonetheless, it is not essential.
Possibly, NS2 prevents an uncontrolled accumulation of viral RNA and
proteins leading to host cell death. It is not clear whether mature
NS2, a precursor protein, e.g., NS2-NS3, or both could account for this
function. Alternatively, the NS2 gene might act at the RNA level,
either by altering the secondary structure or by binding modulating factors.
The CP replicons described here correspond in their overall genome
structure to the naturally occurring defective CSFV RNAs (12, 14,
17, 30), which carry a large deletion comprising most of or the
complete Npro gene, and the coding sequences for all
structural proteins, p7, and NS2. We report an additional CP CSFV RNA
(A187-4263), which by analogy to the BVDV replicon CP9 (1,
16), contains the complete Npro gene. Remarkably,
three different genes with no sequence homology, namely,
Npro, murine ubiquitin, and NS3, are located directly
downstream of the translation start signal of the respective CP
replicons A187-4263, A187-4764Ubi, and A187-4764. This
supports our earlier suggestion that the internal ribosome entry site
of CSFV Alfort/187 does not overlap with the ORF (30) but is
in contrast to what has been reported for CSFV strain C (24)
and for BVDV strains NADL (22) and CP9 (1). Upon
coelectroporation with a full-length marker genome, the CP replicons
were packaged efficiently by the structural proteins provided in
trans from a helper genome, giving rise to CP CSFV (Table
2). Analysis of the NCP replicons revealed detectable amounts of
packaged RNA for A187-Apa but not for A187-E2 and A187-3390.
This is not surprising since the transfection efficiencies of the
latter two RNAs are very low when compared to A187-Apa (Fig. 2). The
RT-PCR data (Fig. 7) further indicate that the replicons propagated in
the presence of helper virus retained their overall genome structure
upon passage, although minor mutations cannot be ruled out. We consider
that the transfection efficiency rather than a specific signal on the
RNA is critical for the packaging of the replicons described here.
Future studies will aim at a more detailed characterization of NS2 and its role in viral replication. Also, CSFV replicons packaged in virions provided in trans from a heterologous expression system will allow helper virus-free experiments. Finally, CSFV replicons may serve as a model for the investigation of hepatitis C virus replication in cell culture.
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ACKNOWLEDGMENTS |
|---|
We thank Michel Baur for the construction of pA187-Apa, Markus
Gerber for excellent technical assistance, C. Mittelholzer for critical
comments, and C. Griot for continuous support.
This work was supported by the Swiss Federal Veterinary Office and the Swiss National Science Foundation (grant 31-46933.96).
| |
FOOTNOTES |
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* Corresponding author. Mailing address: Institute of Virology and Immunoprophylaxis, CH-3147 Mittelhäusern, Switzerland. Phone: 41 31 848 92 11. Fax: 41 31 848 92 22. E-mail: jon-duri.tratschin{at}ivi.admin.ch.
Present address: Institute of Human Gene Therapy, The Wistar
Institute, Philadelphia, PA 19104-4268.
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REFERENCES |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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) polarity (D).
