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Journal of Virology, May 2001, p. 4226-4238, Vol. 75, No. 9
Department of Molecular Microbiology,
Washington University School of Medicine, St. Louis, Missouri
63110,1 and Department of Microbiology
and Immunology, State University of New York Health Science Center
at Brooklyn, Brooklyn, New York 112032
Received 9 October 2000/Accepted 13 February 2001
An internal ribosome entry site (IRES) mediates translation
initiation of bovine viral diarrhea virus (BVDV) RNA. Studies have
suggested that a portion of the Npro open reading frame
(ORF) is required, although its exact function has not been defined.
Here we show that a subgenomic (sg) BVDV RNA in which the NS3 ORF is
preceded only by the 5' nontranslated region did not replicate to
detectable levels following transfection. However, RNA synthesis and
cytopathic effects were observed following serial passage in the
presence of a noncytopathic helper virus. Five sg clones derived from
the passaged virus contained an identical, silent substitution near the
beginning of the NS3 coding sequence (G400U), as well as additional
mutations. Four of the reconstructed mutant RNAs replicated in
transfected cells, and in vitro translation showed increased levels of
NS3 for the mutant RNAs compared to that of wild-type (wt) MetNS3. To
more precisely dissect the role of these mutations, we constructed two
sg derivatives: ad3.10, which contains only the G400U mutation, and
ad3.7, with silent substitutions designed to minimize RNA secondary
structure downstream of the initiator AUG. Both RNAs replicated and
were translated in vitro to similar levels. Moreover, ad3.7 and ad3.10,
but not wt MetNS3, formed toeprints downstream of the initiator AUG
codon in an assay for detecting the binding of 40S ribosomal subunits and 43S ribosomal complexes to the IRES. These results suggest that a
lack of stable RNA secondary structure(s), rather than a specific RNA
sequence, immediately downstream of the initiator AUG is important for
optimal translation initiation of pestivirus RNAs.
The pestiviruses are animal
pathogens causing acute, chronic, and persistent infections that can
result in substantial economic losses in the livestock industry
(22, 31, 41). Members include bovine viral diarrhea virus
(BVDV), classical swine fever virus (CSFV), border disease virus, and
the newly proposed member, BVDV-2 (4). The pestiviruses
are grouped in the Flaviviridae family along with the
hepaciviruses (hepatitis C viruses [HCVs]) and classical
flaviviruses; however, similarities in genome organization, translation
initiation strategy, and polyprotein processing suggest that the
pestiviruses and HCVs are more closely related to each other than to
the classical flaviviruses.
The Flaviviridae are small, enveloped viruses containing a
single-stranded positive-sense RNA genome (31). The
genomes are usually between 9.5 and 12.5 kb in length, with 5' and 3'
nontranslated regions (NTRs) flanking one long open reading frame
(ORF), and lack the 3' poly(A) tract. Translation of the viral RNA
yields a single polyprotein that is co- and posttranslationally
processed by host and viral proteases. The classical flaviviruses
contain a type 1 cap at the 5' end that directs translation initiation in a cap-dependent manner. In contrast, the 5' NTRs of the pestiviruses and HCVs contain structurally and functionally similar internal ribosome entry site (IRES) elements that mediate translation in a
cap-independent manner (reviewed in reference 16).
The first protein of the pestivirus ORF, Npro, is a
nonstructural autoprotease unique to the pestiviruses, which
autocatalytically generates its own C terminus (34). It is
followed by the structural proteins (C, Erns, E1, and E2)
and the nonstructural proteins (p7, NS2-NS3, NS4A, NS4B, NS5A, and
NS5B) (reviewed in reference 22). NS3 harbors serine
protease, helicase, and NTPase activities (37, 38, 44-46), and NS5B exhibits RNA-dependent RNA polymerase activity (48). The identification of these activities implies that
both NS3 and NS5B are directly involved in viral RNA replication.
Two biotypes can be distinguished following infection of cultured
cells. Viruses that do not appear to cause any cell damage are
considered noncytopathic (ncp), whereas cytopathic (cp) isolates cause
cell shrinkage, membrane blebbing, and cell death (22). For BVDV, only unprocessed NS2-NS3 is observed in ncp isolates. In
contrast, production of a discrete NS3 protein in addition to
unprocessed NS2-NS3 has been associated with the cp phenotype. Considerable data suggest that cp viruses usually develop from ncp
viruses by RNA recombination events resulting in genome duplications, rearrangements, deletions, or cellular insertions. However, one report
has demonstrated that single-point mutations in NS2 were responsible
for cytopathic effects (CPE) in the BVDV strain Oregon (14).
Characterization of several isolates revealed that cp BVDV and CSFV
could be composed of RNAs with large internal deletions and an ncp
helper virus (15, 20, 21, 23, 24, 40). In these cases, the
5' NTR and initiating methionine codon were intact, but in-frame
deletions of the structural (C, Erns, E1, and E2) and
nonstructural (p7 and NS2) genes were noted. For simplicity and
continuity, we will refer to these internally deleted genomes as
subgenomic (sg) RNAs (5, 19, 40). The most
well-characterized cp sg BVDV RNA, DI9, has a deletion encompassing all
of the structural proteins as well as p7 and NS2, leaving the C
terminus of Npro fused in frame to NS3 (40).
Additional sg BVDV RNAs have been described, in which portions of
Npro and E1 are fused to NS3 (DI13) (15) or, in others, a
capsid (or NS2)-ubiquitin fusion is inserted between complete or C
terminally truncated Npro and NS3 (3).
However, in most of the sg CSFV RNAs, the initiating AUG codon is fused
in frame to the N terminus of NS3 (21, 24).
Following the identification of the cytopathic sg RNAs, several
investigators created cDNA copies to study the molecular requirements of pestivirus replication and cytopathogenicity (5, 20, 23, 25,
39). The first was based on the DI9 genome, and the derived RNA
replicated and caused CPE following cotransfection with an ncp helper
RNA (20). Subsequent studies showed that the structural proteins, as well as p7 and NS2, were dispensable for viral RNA replication and cytopathogenicity since sg DI9-like RNAs replicated autonomously and caused cell lysis (5, 39). It also
appeared that the first 39 nucleotides (nt) downstream of the
Npro AUG codon were required for replication of the sg
DI9-like RNAs, although the specific Npro amino acid (aa)
sequence was not. However, the specific function of these sequences was
not examined. In contrast, the CSFV sg RNAs, which lacked
Npro, replicated efficiently (23, 25).
To create an experimental system to study pestivirus replication, an sg
RNA was constructed based on the sg CSFV genome organization (MetNS3)
by using the National Animal Disease Laboratory (NADL) strain of BVDV.
We present evidence demonstrating that efficient pestivirus translation
initiation correlates with autonomous sg RNA replication. Furthermore,
the data suggest that binding of 40S ribosomal subunits and formation
of 48S ribosomal initiation complexes require a less-structured or less
stable RNA structure downstream of the initiating methionine.
Cells and viruses.
Madin-Darby bovine kidney (MDBK) cells
were generously provided by M. Collett (ViroPharma, Inc.) and were
propagated in supplemented Dulbecco's modified minimal essential
medium (with sodium pyruvate and 10% horse serum) (19).
Cells were maintained at 37°C with 5% CO2.
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.9.4226-4238.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Efficient Translation Initiation Is Required for
Replication of Bovine Viral Diarrhea Virus Subgenomic
Replicons
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
NADL viruses were
propagated in MDBK cells as previously described (19).
Plasmids.
Plasmids pACNR/NADL and
pACNR/cInsNADL, representing the cp and ncp infectious
cDNAs, respectively, have been described previously (19).
The discistronic reporter plasmid, T7DC1-341, was kindly provided by A. Siddiqui (43). It contained a T7 promoter directing transcription of chloramphenicol acetyltransferase (CAT) and an HCV
IRES driving expression of luciferase (LUC).
NADL, or MetNS3 DNA
sequences (see below) as indicated.
An XbaI site was created upstream of the T7 promoter in
pACNR/NADL (19) as follows. First, a MunI
(T4)-XhoI fragment of pACNR/DraIII
was replaced with an XbaI (T4)-XhoI fragment from
pTet/BVD5'3' (46), regenerating the XbaI site
in pACNR1180/DraIII/BVD5'. Second, an
HaeII-XhoI fragment from
pACNR1180/DraIII/BVD5' was subcloned into
those sites in pACNR/NADL, creating pxNADL.
The pxcInsNADL derivative (I. Frolov and C. M. Rice,
unpublished data) was created by replacing the
NheI-BglII fragment in pxNADL (NADL nt 4930 to
5644) with the corresponding fragment from pACNR/cInsNADL
(nt 4930 to 5374).
For the sg MetNS3 cDNA that is referred to as the wild type (wt),
pMetNS3, the NADL sequence between nt 389 and 5422 was deleted using
recombinant PCR. Oligodeoxynucleotides 183 and 184 were used to amplify
nt 1 to 388, and the 378 and 344 oligodeoxynucleotides amplified nt
5423 to 5835 (Table 1).
Oligodeoxynucleotide primers 378 and 379 contained an ATG codon and a
silent nucleotide change (bold), creating an ApaI site
(underlined) at the deletion breakpoint (Table 1). The PCR-amplified
fragments were digested with ApaI and then ligated, and the
product was digested with XhoI-BglII. This
fragment was used to replace the corresponding
XhoI-BglII fragment (nt 224 to 5644) in
pACNR/NADL (Fig. 1).
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22 to
434) was subcloned into those sites in wt pxMetNS3.
The initial cDNA copy of adapted MetNS3 RNA was obtained by reverse
transcription-PCR (RT-PCR) of MetNS3 RNA isolated from the supernatant
of cells infected with passage 4 virus (cInsNADL and
MetNS3). To create pxMetNS3ad3, a portion of the RT-PCR product was
digested with SphI and BglII and subcloned into
those sites in pxNproNS3, as described above. Five
individual cDNA clones (ad3.1, ad3.2, ad3.4, ad3.5, and ad3.6) were
sequenced and used for further investigation (see Results).
In vitro transcription of RNA.
Plasmid DNAs containing
full-length and sg BVDV NADL sequences were digested with
SdaI, and the reporter plasmid, T7DC1-341, was digested with
HpaI (LUC expression, transfection studies) or
SalI (CAT expression only, in vitro translation). The
linearized DNAs were extracted with phenol-chloroform (1:1) and
chloroform alone and then were precipitated with ethanol. Pelleted DNAs
were resuspended in double-distilled water (ddH2O) and
transcribed in vitro using the T7-MEGAscript kit (Ambion, Austin, Tex.)
in the presence of 1 µCi of [3H]UTP (Dupont NEN,
Boston, Mass.), as recommended by the manufacturer (19).
The in vitro-synthesized RNAs were resuspended in ddH2O at
approximately 1 µg/µl based on [3H]UTP incorporation.
Transcript RNAs and standard RNAs of known concentrations were
separated on a 1% agarose gel and stained with ethidium bromide. The
final RNA concentrations were determined using a Fluorimager (Molecular
Dynamics, Sunnyvale, Calif.) in conjunction with the IPLab
Gel program (Scantalytics, Inc., Fairfax, Va.). RNA aliquots were
stored at 80°C.
Transfection of cultured cells.
Transfection of MDBK cells
by electroporation was performed essentially as described previously
(19). Briefly, MDBK cells (approximately 80% confluent)
were detached by trypsin treatment; washed three times in sterile,
ice-cold phosphate-buffered saline (PBS); and resuspended at between
1.0 × 107 and 2.0 × 107 cells/ml in
PBS. Volumes containing 4 to 5 µg of full-length or sg RNA
transcripts were combined with 1 µg of LUC reporter RNA (DCI-341),
mixed with 0.4 ml of washed MDBK cells, and pulsed immediately (1.5 kV,
25 µF, 
resistance, and 2 pulses) using a Bio-Rad Gene Pulser
(Hercules, Calif.). The total RNA transfected per reaction mixture was
equalized using uninfected MDBK cellular RNA that had been extracted
using TRIzol reagent (Gibco-BRL, Grand Island, N.Y.) as described
below. The pulsed samples were diluted to 10 ml with Dulbecco's
minimal essential medium (supplemented with 10% horse serum and sodium
pyruvate), added to either a 100-mm-diameter dish or split equally into
four 35-mm-diameter wells, and incubated at 37°C with 5%
CO2. The specific infectivity of full-length RNA was
determined using an infectious center assay as described previously (19).
NADL (multiplicity of infection [MOI] = ~2)
and splitting the infected cells once prior to superinfection. The
cells were incubated at 37°C with 5% CO2 until CPE was
observed. CPE was noted usually 24 to 48 h following
superinfection, and the passage on persistently infected MDBK cells was
repeated. Significant levels of CPE were present by passage 4 in the
superinfected cells, at which point the cell supernatants were
collected, clarified, and stored at 80°C as a passage 4 virus stock.
Protein analysis. Transfection efficiency was monitored in the transfected cells by quantitation of LUC activity at 8 h posttransfection (p.t.). Cell monolayers (35-mm-diameter wells) were washed twice with PBS and resuspended in 250 µl of 1% Triton X-100 lysis buffer (25 mM Tris-HCl, pH 7.5; 25 mM dithiothreitol; 2 mM EGTA; 1% [vol/vol] Triton X-100). The LUC activity in one-tenth of the clarified cell extract was measured using a luminometer (EG&G Berthold, Gaithersburg, Md.).
For Western blot analysis, cell lysates from 35-mm-diameter wells were prepared in 300 µl of 0.5% sodium dodecyl sulfate (SDS) lysis buffer (50 mM Tris-HCl, pH 7.5; 150 mM NaCl; 0.5% SDS; 20 µg of phenylmethylsulfonyl fluoride/ml; 1 µg of aprotinin/ml) at the times p.t. indicated in the figure legends. Total protein concentration was determined using the bicinchonic acid protein assay (Pierce, Rockford, Ill.) as recommended by the manufacturer except that all volumes were reduced by one-half. Equivalent amounts of total protein were analyzed by immunoblotting with polyclonal rabbit NS3-specific antisera (G40) following protein separation by SDS-8% polyacrylamide gel electrophoresis (PAGE), as described previously (19). Subsaturating concentrations of T7-transcribed sg RNAs (data not shown) were translated in vitro using rabbit reticulocyte lysates (Promega; Madison, Wis.) in the presence of [35S]methionine (Amersham, Piscataway, N.J.). Each translation reaction mixture contained CAT mRNA in addition to the indicated sg RNA for subsequent normalization of the NS3 translation levels. Samples were diluted 10-fold in Laemmli sample buffer and analyzed by SDS-9% PAGE. The radiolabeled bands were detected by autoradiography and quantitated with a Molecular Imager (Bio-Rad Laboratories).Viral RNA analysis.
Initially, RNA synthesis and
accumulation were examined by [3H]uridine (30 µCi/m)
(ICN Biomedicals, Inc., Costa Mesa, Calif.) incorporation in the
presence of dactinomycin (1 µg/ml) (Fig. 2). Alternatively, 200 µCi of
[32P]orthophosphate
(H332PO4)/ml was added during the
exponential phase of sg RNA synthesis in media containing low levels of
phosphate at concentrations that yielded NADL viral titers between 50 and 80% of those obtained in complete media (data not shown). RNAs
from the transfected, radiolabeled cells were isolated using TRIzol
reagent (Gibco-BRL). To ensure recovery of total RNA, detached cells
were collected from the supernatants by low-speed centrifugation and
the pelleted cells were combined with the corresponding monolayer
lysate. RNAs were isolated according to the manufacturer's protocol,
except that carrier tRNA (25 µg) was added to each lysate and an
additional chloroform extraction was performed.
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Assembly and analysis of ribosomal and ribonucleoprotein complexes. Ribosomal subunits, subunit of eukaryotic initiation factor 2 (eIF2) and eIF3 were purified from rabbit reticulocyte lysates (Green Hectares, Oregon, Wis.) as previously described (28, 29). Ribosomal complexes and complexes between BVDV mRNA and eIF3 were assembled on BVDV mRNA, essentially as previously described (27). BVDV plasmids were linearized with BglII, and mRNAs were transcribed in vitro using T7 RNA polymerase. Aliquots of the mRNAs (0.6 µg) were incubated for 5 min at 30°C in a 40-µl reaction volume that contained 0.4 mM GMP-PNP, Met-tRNAiMet (6 pmol), 40S subunits (6 pmol), eIF2 (3 µg), and eIF3 (7 µg) as indicated in the text. [35S]methionine-labeled Met-tRNAiMet was prepared using rabbit tRNA (Novagen, Madison, Wis.) and aminoacyl-tRNA synthetase purified from Escherichia coli MRE600 (American Type Culture Collection, Manassas, Va.), as described previously (28).
Ribosomal and RNP complexes were analyzed by primer extension (28), using primer 5'-GTAAGCTCGTAGGGAACC-3' (complementary to nt 5541 to 5558 of the BVDV genomic sequence) and avian myeloblastosis virus reverse transcriptase (Promega) in the presence of [
-32P]dATP (~6,000 Ci/mmol) as
described. The cDNA products were ethanol precipitated, resuspended,
and analyzed by electrophoresis through 6% polyacrylamide sequencing
gels. The cDNA products were compared with appropriate
dideoxynucleotide sequence ladders.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Adaptive mutations are required for replication of sg NADL MetNS3
RNA in cell culture.
To study the genetic requirements of
pestivirus replication and cytopathogenicity, we created a classical
swine fever-like sg cDNA (MetNS3) derived from an infectious NADL cDNA
clone. For MetNS3, the complete NADL 5' NTR and initiating methionine
codon were fused in frame with the first codon of NS3
(14), which was contiguous with the remainder of the NADL
sequence (19). MDBK cells were cotransfected with in
vitro-synthesized sg MetNS3 and ncp cInsNADL RNAs (Fig.
1) and observed for the development of CPE (19). Surprisingly, neither CPE nor sg RNA replication was detected in the
transfected cells, whereas replication of ncp cInsNADL
virus was readily observed (data not shown). Identical results were
obtained after transfection of MetNS3 RNA into persistently infected
MDBK cells. However, if the extracellular supernatant was serially
passaged on persistently infected MDBK cells, significant CPE was
eventually observed (data not shown). Similar to results reported for
another virus stock containing both sg and full-length RNA (CP13), the
number of PFU was 10- to 100-fold lower than the number of
focus-forming units in the passaged virus stocks (15). Thus, the range of MOIs that could be reasonably achieved in subsequent infections was limited.
NADL and sg MetNS3
RNAs were observed in infected cell extracts but not in mock-infected
cell extracts (Fig. 2A, lanes 1 and 2, respectively). Moreover,
replication of the sg MetNS3 RNA was associated with the appearance of
CPE (Fig. 2B). These results suggest that either the sg RNA, the ncp
helper RNA, or both accumulate adaptive changes during serial passage.
Adaptive mutations in the ncp cInsNADL RNA were less
likely based on our data showing that this virus remains noncytopathic
during passage (data not shown). These data also show that the MetNS3
RNA could be packaged in trans by the ncp
cInsNADL helper virus present in the persistently
infected MDBK cells.
To determine if the passaged sg MetNS3 RNAs contained adaptive
mutations, the RNA population in the passage 4 virus stock was
amplified by RT-PCR and sequenced. Mutations specific for the sg RNA
population were mapped using primers that amplified the MetNS3
junction. Although nt 1 to 2568, which includes the 5' NTR (nt 1 to
385), NS3 gene (nt 386 to 2437), and the N-terminal two-thirds of NS4A
(nt 2438 to 2629) were sequenced, only a single silent nucleotide
substitution (G400U) at the beginning of the NS3 was identified
(initiator AUG at nt 386 to 388). To determine if the silent G400U
mutation or other less frequent mutations were sufficient to facilitate
RNA replication and CPE, we replaced the corresponding wt MetNS3
SphI-BglII fragment (nt 247 to 610) with the
mutant RT-PCR product.
Automated sequence analysis of the SphI-BgII
fragment of five individual cDNA clones (ad3.1, ad3.2, ad3.4, ad3.5,
and ad3.6) revealed at least one additional mutation in each clone
(Fig. 3A), with the additional mutation
in ad3.2 (A460C) also silent, thereby creating a mutant without any
amino acid changes. Clone ad3.6 contained two mutations in common with
ad3.5 as well as an additional downstream amino acid substitution,
suggesting a common RNA ancestor. The additional mutations not detected
by direct sequencing of the RT-PCR products may represent minor
variants in the population.
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)
transfections (lanes 1) lacked RNA. RNA accumulation was detected by
radiolabeling the transfected cells with
H332PO4 between 16 and 24 h p.t. in
the presence of dactinomycin. Total cellular RNA was glyoxylated,
separated on a 1% agarose gel, and visualized by autoradiography. The
position of the sg RNA is indicated. The radiolabeled bands were
quantitated with a Molecular Imager (Bio-Rad Laboratories) and
normalized to transfection efficiency and total 18S rRNA as described
in Materials and Methods. The percentages of each sg RNA relative to
ad3.4 (100%) are indicated. (B). Transfected cell lysates were
prepared at 18 h p.t. and separated by SDS-8% PAGE. NS3 levels
were detected with polyclonal rabbit NS3-specific antisera by Western
blot analysis. Molecular mass markers are indicated on the right and
the migration of NS3 is indicated on the left (C).
Adapted ad3 RNA replicate autonomously. Recent reports demonstrated that an sg BVDV DI9 RNA could replicate autonomously in cultured cells and was able to induce CPE in the absence of an ncp helper virus (5, 39). The sg DI9 or DI9-like RNAs do not encode structural proteins. Thus, viral packaging, release, and spread were absent, and RNA replication and cytopathogenicity were examined as first-cycle events in transfected cells. To determine if the reconstructed sg MetNS3 RNAs were capable of autonomous replication, MDBK cells were transfected with in vitro-synthesized RNA and a LUC reporter RNA as a transfection control (43). Transfected cells were split into 35-mm-diameter wells to examine viral RNA accumulation, protein expression, CPE, and LUC activity.
Cells transfected with the mutant sg RNAs ad3.1, ad3.2, ad3.4, and ad3.5 developed CPE that included vacuole formation, cell shrinkage, and detachment and were distinguishable from that induced by dactinomycin treatment alone (data not shown). Accumulation of 32P-labeled sg RNA was observed for ad3.1, ad3.2, ad3.4, and ad3.5 (Fig. 3B, lanes 3, 4, 5, and 6), whereas neither in vivo-labeled ad3.6 RNA nor wt MetNS3 RNA was detectable under these conditions. RNA accumulation in ad3.4-transfected cells was reproducibly higher than it was in the others and was set at 100% for quantitation comparisons with other samples (see Materials and Methods). The levels of accumulated ad3.1 and ad3.2 RNAs were somewhat reduced (83 and 51% of that of ad3.4, respectively; Fig. 3B, lanes 3 and 4), whereas the level of ad3.5 was significantly lower (29%; Fig. 3B, lane 6). As expected, the mock- and wt MetNS3-transfected cells did not show detectable accumulation of discrete 32P-labeled RNA products (Fig. 3A, lanes 1 and 2). In vivo-labeled 32P-labeled RNAs comigrated with in vitro-synthesized MetNS3 sg RNA transcripts (data not shown). These data demonstrate that two silent mutations in the ad3.2 RNA are sufficient for autonomous replication and CPE (Fig. 3B, lane 4), and it is likely that the prevalent G400U substitution is important for replication. Furthermore, the additional mutation in ad3.6 was probably detrimental to NS3 activity. To examine polyprotein synthesis and processing, transfected cell extracts were analyzed for NS3 protein levels by Western blotting (7, 19). All replication-competent sg RNAs expressed NS3 (Fig. 3C, lanes 3, 4, 5, and 6) and the level of NS3 expression correlated with the level of RNA accumulation. Furthermore, NS3 expressed from the replicons comigrated with NS3 produced in NADL virus-infected cells (data not shown). In the absence of detectable replication, primary translation of the input transcripts did not produce detectable levels of NS3 (Fig. 3C, lanes 2 and 7). Moreover, a lack of unprocessed polyprotein precursor containing NS3 indicated that the NS3-NS4A site was efficiently processed in the replicons and demonstrated the presence of an active NS3 protease (Fig. 3C, lanes 3, 4, 5, and 6). Based on these data, we hypothesized that the silent mutations in the protein coding sequence could be affecting a cis element required for RNA replication or perhaps a step prior to replication, such as translation. To address these possibilities, we first examined primary translation in a cell-free system independent of replication.Translation of wt MetNS3 RNA in vitro is reduced compared to
adapted MetNS3 RNAs.
To analyze the effect of the wt and mutant
NS3 sequences on NADL IRES function, the sg MetNS3 RNAs were translated
in vitro in the presence of [35S]methionine to detect the
proteins. The level of NS3 translated from each RNA was normalized by
comparing the amount of NS3 to the level of CAT expressed from a
separate transcript (see Materials and Methods). As shown in Fig.
4, the level of 35S-labeled
wt NS3 was between 8- to 10-fold less than the levels of adapted NS3,
suggesting that there was a defect in the translation initiation of wt
MetNS3 (Fig. 4, compare lane 3 with lanes 4, 5, 6, 7, and 8). In
contrast, translation of ad3.6 NS3 appeared similar to that of NS3
expressed from the replicating sg RNAs, suggesting that the inability
of ad3.6 to replicate may be due to an impairment in NS3 function and
not to reduced translation initiation (Fig. 4, compare lane 8 to lanes
4, 5, 6, and 7). As controls, we confirmed that the in
vitro-synthesized NS3 proteins comigrated with authentic NS3 from
NADL-infected cells (data not shown) and that no
35S-labeled protein products were observed in the mock
reaction mixture (Fig. 4, lane 1).
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Type 2 IRES-mediated translation initiation allows replication of wt MetNS3 RNA. If the lack of detectable wt MetNS3 RNA replication was due to reduced translation, increasing translation efficiency should enhance replication. On the other hand, if wt MetNS3 lacks a cis-acting replication signal or inhibits RNA synthesis directly, increasing the level of translation should not significantly influence sg RNA replication. To distinguish between these possibilities, the wt MetNS3 5' NTR was replaced with a chm BVDV-EMCV 5' NTR that contained the three 5' terminal BVDV hairpins required for BVDV replication (Fig. 5A) fused to the canonical EMCV IRES element (9). Since the EMCV IRES functions independently of sequences downstream of the initiator methionine codon (12), chm MetNS3 RNA would allow us to determine the effect of the wt MetNS3 coding sequences on RNA replication independently of translation.
In vitro, chm MetNS3 was translated efficiently and at levels twofold higher than those of the adapted sg RNAs (data not shown). Replication of chm MetNS3 RNA was assayed following transfection of MDBK cells, and similar levels of 32P-labeled sg RNAs were detected for chm MetNS3 and ad3.1 (Fig. 5B, compare lane 4 with lane 3). Furthermore, replication of the sg RNAs was associated with cytopathology in the transfected cell monolayers (data not shown). These results demonstrate that wt MetNS3 does not have a cis-acting RNA replication defect, suggesting that inefficient translation may be limiting wt MetNS3 replication.
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MetNS3 RNAs with less-stable RNA structures downstream of the AUG codon replicate efficiently. It was possible that the nucleotide sequence or RNA structure downstream of the AUG codon in wt MetNS3 inhibited translation initiation, similar to that reported for HCV IRES-driven translation (10, 11). The 5' NS3 sequence in wt MetNS3 is GC-rich (Fig. 3A) and might predispose this region to form a stable RNA structure. In keeping with this hypothesis, the NS3 sequence downstream of the initiator methionine in the replication-competent sg CSFV MetNS3 RNAs is AU-rich and the nucleotide at position 400 is a U (21).
To address this possibility, we created a MetNS3 RNA with a predicted less-stable or unstructured RNA element downstream of the AUG codon having silent A or U substitutions at the third base position of the second, third, fourth, fifth, seventh, and eighth NS3 codons (Fig. 6A; ad3.7). Two additional MetNS3 cDNAs were also constructed: ad3.8 (Fig. 6A, C394U [ApaI site]), to determine if the silent U394C substitution created during the engineering of wt MetNS3 was responsible for the replication-defective phenotype, and ad3.10 (G400U), to test if the prevalent G400U mutation alone was sufficient for translation and autonomous replication (Fig. 6A).
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G of 11.5
and 11.6 kcal/mol at 37°C, and three stem-loops with similar
thermodynamic stability, with G from 11.0 to 11.6
kcal/mol, were formed for ad3.8 (predicted stem-loop shown in Fig. 9).
In contrast, ad3.7 and ad3.10 formed four and five stem-loop
structures, respectively, with significantly less-stable structures
(G = 3.7 to 4.6 kcal/mol and 4.9 to 5.6
kcal/mol at 37°C, respectively). Due to the region folded, the
remaining replicons and ad3.6 had the same structures and stability as
ad3.10. Consistently, the G400U substitution in the replicons and
ad3.10 disrupted base pairing in the stem, which was associated with
decreased thermodynamic stability of the stem-loop structure. For
ad3.7, the multiple substitutions disrupted the basic structure of the
stem-loop, with the U at position 400 being paired in some cases and
unpaired in others.
Structure-probing experiments of the RNA region surrounding the
initiator AUG in wt MetNS3, ad3.7, and ad3.10 were performed by mapping
the RNase T1- and RNase V1-sensitive bases.
Although our results were not conclusive, the data did suggest enhanced RNase T1 sensitivity at nt 402 in the ad3.7 and ad3.10
RNAs, consistent with the hypothesis that these RNAs may contain less
structure downstream of the initiating methionine (data not shown).
To determine if the RNAs with predicted less-stable secondary
structures would replicate autonomously, the sg MetNS3 RNAs were
synthesized in vitro from the engineered cDNA templates and transfected
into MDBK cells, and RNA replication was measured by incorporation of
32P as described previously. Both the AU-rich RNA (ad3.7)
and the RNA containing the single adaptive G400U (ad3.10) substitution replicated efficiently, as demonstrated by the accumulation of distinct
32P-labeled RNAs (Fig. 6B, lanes 8 and 10). In contrast,
the single U394C change was not responsible for repressed replication
since ad3.8 did not accumulate detectable levels of
32P-labeled RNA (Fig. 6B, lane 9). These results show that
sg RNAs with predicted less-stable RNA secondary structures (ad3.7 and ad3.10) downstream of the AUG replicate autonomously and that the G400U
substitution alone is sufficient.
As expected, ad3.7 and ad3.10 showed similar levels of NS3 protein
synthesis in vitro (55 and 65% of the level of ad3.4 NS3, respectively), whereas ad3.8 NS3 levels were consistently less than
30% of that of ad3.4 (data not shown). These data show that sg RNAs
that translate efficiently in vitro replicate efficiently and that
reduced translation in vitro correlates with undetectable levels of RNA
replication in transfected MDBK cells.
Adapted MetNS3, but not wt MetNS3, binds 40S ribosomes and forms 48S ribosomal initiation complexes. Translation initiation of BVDV, CSFV, and the related HCV has been evaluated in vitro using purified translation components and in vitro-transcribed RNAs (27, 29). Therefore, to analyze the efficiency of IRES-mediated translation initiation in the wt MetNS3, ad3.7 (AU-rich), and ad3.10 (G400U) RNAs, we reconstituted this process in vitro to the stage of 48S initiation complex formation. The ribosomal complexes were analyzed by toeprinting, which involves primer extension by reverse transcriptase on a template RNA to which a protein or ribosomal complex is bound. Synthesis of the cDNA is arrested at the leading edge of the complex, yielding toeprints that can be accurately mapped on sequencing gels.
The BVDV IRES is highly structured (see Fig. 8), and as a result, reverse transcriptase arrest occurs at several sites even in the absence of translation components. Three of these sites occur on wt genomic BVDV mRNA (27) and also on wt MetNS3 and adapted variant RNAs (at A320, G327, and U352; Fig. 7, lanes 1, 5, and 9). Prominent reverse transcriptase stops were also detected at GCCG (nt 395 to 398) on wt MetNS3 and ad3.10 RNAs (Fig. 7, lanes 1 and 9), indicative of a stable secondary structure at or immediately upstream of these residues. Corresponding stops on ad3.7 RNA were less intense, indicating that the ad3.7 mRNA is less structured downstream of the initiation codon (Fig. 7, lane 5).
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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In this study, we created an sg NADL RNA (MetNS3) based on the genome structure of the cp CSFV isolates, in which the 5' NTR and initiating AUG codon were fused to the N terminus of NS3 (Fig. 1; 21, 23). In contrast to earlier reports in the literature for sg CSFV RNA of similar structure, neither replication nor induction of CPE was observed for sg NADL MetNS3. However, following serial passage in the presence of ncp helper virus, detectable sg RNA replication and CPE were detected (Fig. 2). These results suggested that perhaps the Npro sequence was essential, similar to reports for the BVDV DI9-like RNAs (5, 39). However, efficient replication of the reconstructed RNAs, ad3.1, ad3.2, ad3.4, and ad3.5 (Fig. 3A and B, lanes 3 to 6), showed that a specific Npro nucleotide or amino acid sequence was not required. Furthermore, comparison of the Npro and NS3 sequences over the first 114 nt (38 aa) revealed very little homology at the nucleotide (29 to 31% identity) or amino acid (8 to 10.5% identity) level.
The combined results of reduced wt MetNS3 translation in vitro (Fig. 4, lane 3) and autonomous replication of the 5' NTR chimera RNA, chm MetNS3 (Fig. 5B, lane 4), suggested that the sequences downstream of the initiating AUG codon were directly influencing BVDV IRES-directed translation initiation and not RNA synthesis. This conclusion is not unprecedented since translation initiation directed by the BVDV or closely related HCV IRES elements has been reported to require downstream sequences within the 5' portion of the ORFs (6, 11, 17, 30). In contrast, others have reported efficient HCV IRES-directed translation in the absence of HCV coding sequences (32, 42, 43). Honda et al. (10) suggested that the conflicting reports for HCV IRES-mediated translation were due to a stable RNA secondary structure near the initiating AUG codon, because mutations which increased the stability of the stem-loop surrounding the HCV initiator AUG codon were inversely correlated with translation efficiency.
In support of the latter ideas, we observed that sg RNAs (ad3.1, ad3.2, ad3.4, ad3.5, ad3.7, and ad3.10) that were predicted to have less-stable RNA secondary structures near the AUG codon were able to translate (Fig. 4, lanes 4 to 7, and data not shown) and replicate efficiently (Fig. 3, lanes 3 to 6; Fig. 6, lanes 3 to 6, 8, and 10). In contrast, sg RNAs (wt MetNS3 and ad3.8) with secondary structures predicted to be more stable were translated poorly (Fig. 4, lane 3, and data not shown) and did not replicate to detectable levels (Fig. 3B, lane 2; Fig. 6B, lanes 2 and 9). Furthermore, enhanced RNase T1 cleavage at nt 402 was observed in the replication-competent sg RNAs of ad3.7 and ad3.10, with the prevalent G400U substitution, but not in wt MetNS3 RNA. These data suggest that the presence of a U at nt 400 may promote formation of an RNase T1-accessible, single-stranded RNA in this region. The inability of ad3.6 to replicate to detectable levels, even though it was translated efficiently (Fig. 4, lane 8), may have been due to the influence of the additional amino acid mutation on NS3 function (R51S; Fig. 3A).
Our data do not preclude the possibility that additional RNA-protein interactions modulate BVDV-IRES-mediated translation initiation in vivo. However, the inability of the 40S ribosomal subunits and 43S complexes to bind wt MetNS3 RNA in vitro provides strong evidence that the wt MetNS3 RNA inhibits translation initiation through an intrinsic property of the RNA (Fig. 7, lanes 2 and 3). Furthermore, base substitutions which are predicted to decrease the thermodynamic stability of RNA structures within this region allowed 40S binding and subsequent 48S complex formation, albeit at different levels for ad3.7 and ad3.10 (Fig. 7, compare lanes 6 and 7 with 10 and 11). Although the ad3.10 RNA was significantly less efficient at binding 40S ribosomal subunits and 43S ribosomal preinitiation complexes in vitro than ad3.7, the levels of sg RNA replication in cultured cells were similar (Fig. 6, lanes 8 and 10).
The binding of 40S ribosomal subunits to pestivirus and HCV IRES elements closely resembles the mechanism of 30S ribosomal subunits binding to prokaryotic mRNAs (13, 27, 29). In prokaryotes, the 30S ribosome binding site is extremely sensitive to the presence of stable RNA secondary structures, such that small increases in stability (2.4 kcal/mol) can decrease binding by an order of magnitude (reviewed in reference 8). Hence, it appears that the stability of the RNA secondary structure at the 30S ribosome binding site is quite close to the threshold for being inhibitory. Our results are consistent with the observation that increased RNA secondary structure can significantly inhibit ribosome binding and that a single G-to-U substitution predicted to decrease the stability of the RNA secondary structure permitted 40S ribosome binding.
It is also possible that either an A or C at position 400 would have
allowed translation and sg RNA replication. The translation and
autonomous replication of ad3.7 suggest that the identity of the
primary sequence, at least at the third base position, is not as
important as the resulting effects on secondary structure. This
hypothesis is compatible with the observation that changes in RNA
secondary structure have a far greater impact on 30S ribosome binding
than the identity of the specific nucleotide substitution (8). The predicted stability of RNAs with either an A or C at nt 400 (G between 6.5 and 8.0 kcal/mol) was
increased relative to that of ad3.10 and ad3.7 but less than that of wt
MetNS3 or ad3.8. Since our results suggested that the thermodynamic
threshold (G) for 40S binding to the MetNS3 RNA is
between 5.6 and 11.0 kcal/mol, it will interesting to determine the
effect of the A and C substitutions at position 400.
Another explanation is that within the cellular milieu, additional host factors influence translation initiation. Several studies have demonstrated interactions between La protein and polypyrimidine tract binding protein (PTB) with the related HCV IRES element (reviewed in reference 16). La protein specifically interacts with the HCV RNA in the context of the initiator methionine codon and may contribute to efficient translation initiation (1, 2). La protein is an RNA binding protein with helicase activity and, hence, may unwind double-stranded RNA in preparation for translation initiation. In addition, La has been shown to associate with small ribosomal subunits in the cytoplasm (26). The possible role(s) of PTB in HCV IRES-mediated translation initiation is somewhat less definitive but may involve PTB acting as an RNA chaperone or perhaps through additional protein-protein interactions (16). For BVDV, recent results have shown that although PTB weakly binds BVDV IRES RNA, it does not influence BVDV IRES-mediated translation in vitro (36). Therefore, it is possible that La or other, as-yet-unidentified cellular proteins influence BVDV IRES-directed translation initiation.
The importance of maintaining wt BVDV 5' Npro sequence for efficient replication was supported by the observation that at least 28 aa of Npro were found in 11 sg RNAs isolated from four different animals (3). Our data are also consistent with the results obtained with the D19-like replicons, for which a portion of Npro was necessary for sg RNA replication (5, 39). Efficient translation initiation, including 40S and 43S binding, was associated with sg RNA replication, and since translation was not examined in the nonreplicating DI9-like RNAs, it is entirely possible that they were defective in protein synthesis.
These data and those of others (10, 11, 13, 13a, 27, 29,
33) led us to propose a model for type 3 IRES-mediated translation initiation (Fig. 9).
Effective binding of the 40S ribosomal subunit to the initiator AUG
codon requires the surrounding RNA to be relatively unstructured (Fig.
9A, left) since stable RNA secondary structure(s) immediately
downstream of the canonical IRES (Fig. 9A, stem-loop, right) appear to
inhibit 40S binding (Fig. 9B). In the absence of 40S binding, 48S
initiation complex formation and subsequent translation initiation are
blocked (Fig. 9C). The ability to influence type 3 IRES-driven
translation initiation by increasing RNA secondary structure downstream
of the initiator AUG codon may have evolved as a mechanism for
controlling viral gene expression and subsequent RNA replication in
virus-infected cells. In addition, translation initiation could be
modulated by binding of viral or host proteins or of both, such that
the stability of the RNA secondary structure is either increased or decreased.
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Taken together, these results also suggest that pestivirus translation and RNA replication are coupled processes in vivo. Similarly, Yu et al. (47) reported that the 5' terminal stem loop of the BVDV IRES contains a cis-acting element involved in regulation of both translation and replication. The inapparent replication of wt MetNS3 RNA in the presence of the ncp helper virus also suggests that complementation of RNA replication does not occur in trans, at least to detectable levels. It is likely that the regulation of translation and replication in vivo is tightly regulated and that BVDV modulates various host responses by controlling viral protein and RNA levels.
In summary, using engineered sg BVDV replicons, we have shown that efficient translation initiation likely requires a less-structured RNA surrounding the AUG initiation codon. Moreover, it appears that certain levels of viral protein expression are necessary to support a complete RNA replication cycle. We have demonstrated interactions of the sg RNAs with the 40S and 43S ribosomal complexes and that the formation of the ribosomal preinitiation complexes associates with biological function in vitro.
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ACKNOWLEDGMENTS |
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We thank Rebecca Moran for expert technical assistance and Tatyana Pestova for advice and reagents. We are also grateful to many colleagues for helpful discussions during the course of this work and to Beate Kümmerer, Keril Blight, Arash Grakoui, Holly Hanson, Jane McKeating, and Sondra Schlesinger for careful reading of the manuscript. We are indebted to Bill Goldman for valuable advice and for providing access to his Fluorimager.
T.M.M. was supported by a fellowship from the U.S. Department of Agriculture (9802328). This work was supported in part by grants from the Public Health Service (CA57973 and AI44118).
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FOOTNOTES |
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* Corresponding author. Present address: Center for the Study of Hepatitis C, The Rockefeller University, Box 64, 1230 York Ave., New York, NY 10021. Phone: (212) 327-7046. Fax: (212) 327-7048. E-mail: ricec{at}rockefeller.edu.
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REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. |
Ali, N.,
G. J. Pruijn,
D. J. Kenan,
J. D. Keene, and A. Siddiqui.
2000.
Human La antigen is required for the hepatitis C virus internal ribosome entry site (IRES)-mediated translation.
J. Biol. Chem.
275:27531-27540 |
| 2. |
Ali, N., and A. Siddiqui.
1997.
The La antigen binds 5' noncoding region of the hepatitis C virus RNA in the context of the initiator AUG codon and stimulates internal ribosome entry site-mediated translation.
Proc. Natl. Acad. Sci. USA
94:2249-2254 |
| 3. |
Becher, P.,
M. Orlich,
M. Konig, and H. J. Thiel.
1999.
Nonhomologous RNA recombination in bovine viral diarrhea virus: molecular characterization of a variety of subgenomic RNAs isolated during an outbreak of fatal mucosal disease.
J. Virol.
73:5646-5653 |
| 4. | Becher, P., M. Orlich, A. Kosmidou, M. Konig, M. Baroth, and H. J. Thiel. 1999. Genetic diversity of pestiviruses: identification of novel groups and implications for classification. Virology 262:64-71[CrossRef][Medline]. |
| 5. |
Behrens, S.-E.,
C. W. Grassmann,
H.-J. Thiel,
G. Meyers, and N. Tautz.
1998.
Characterization of an autonomous subgenomic pestivirus RNA replicon.
J. Virol.
72:2364-2372 |
| 6. | Chon, S. K., D. R. Perez, and R. O. Donis. 1998. Genetic analysis of the internal ribosome entry segment of bovine viral diarrhea virus. Virology 251:370-382[CrossRef][Medline]. |
| 7. | Collett, M. S., R. Larson, S. K. Belzer, and E. Retzel. 1988. Proteins encoded by bovine viral diarrhea virus: the genomic organization of a pestivirus. Virology 165:200-208[CrossRef][Medline]. |
| 8. | de Smit, M. H., and J. van Duin. 1990. Control of prokaryotic translational initiation by mRNA secondary structure. Prog. Nucleic Acid Res. Mol. Biol. 38:1-35[Medline]. |
| 9. | Frolov, I., M. S. McBride, and C. M. Rice. 1998. cis-acting RNA elements required for replication of bovine viral diarrhea virus-hepatitis C virus 5' nontranslated region chimeras. RNA 4:1418-1435[Abstract]. |
| 10. | Honda, M., E. A. Brown, and S. M. Lemon. 1996. Stability of a stem-loop involving the initiator AUG controls the efficiency of internal initiation of translation on hepatitis C virus RNA. RNA 2:955-968[Abstract]. |
| 11. | Honda, M., L. H. Ping, R. C. Rijnbrand, E. Amphlett, B. Clarke, D. Rowlands, and S. M. Lemon. 1996. Structural requirements for initiation of translation by internal ribosome entry within genome-length hepatitis C virus RNA. Virology 222:31-42[CrossRef][Medline]. |
| 12. | Hunt, S. L., A. Kaminski, and R. J. Jackson. 1993. The influence of viral coding sequences on the efficiency of internal initiation of translation of cardiovirus RNAs. Virology 197:801-807[CrossRef][Medline]. |
| 13. |
Kolupaeva, V. G.,
T. V. Pestova, and C. U. Hellen.
2000.
An enzymatic footprinting analysis of the interaction of the 40S ribosomal subunits with the internal ribosomal entry site of hepatitis C virus.
J. Virol.
74:6242-6250 |
| 13a. | Kolupaeva, V. G., T. V. Pestova, and C. U. T. Hellen. 2000. Ribosome binding to the internal ribosome entry site of classical swine fever virus. RNA 6:1791-1807[Abstract]. |
| 14. |
Kümmerer, B. M.,
D. Stoll, and G. Meyers.
1998.
Bovine viral diarrhea virus strain Oregon: a novel mechanism for processing of NS2-3 based on point mutations.
J. Virol.
72:4127-4138 |
| 15. | Kupfermann, H., H.-J. Thiel, E. J. Dubovi, and G. Meyers. 1996. Bovine viral diarrhea virus: characterization of a cytopathogenic defective interfering particle with two internal deletions. J. Virol. 70:8175-8181[Abstract]. |
| 16. | Lemon, S. H., and M. Honda. 1997. Internal ribosome entry sites within the RNA genomes of hepatitis C virus and other flaviviruses. Semin. Virol. 8:274-288[CrossRef]. |
| 17. |
Lu, H. H., and E. Wimmer.
1996.
Poliovirus chimeras replicating under the translational control of genetic elements of hepatitis C virus reveal unusual properties of the internal ribosomal entry site of hepatitis C virus.
Proc. Natl. Acad. Sci. USA
93:1412-1417 |
| 18. | Mathews, D. H., J. Sabina, M. Zuker, and D. H. Turner. 1999. Expanded sequence dependence of thermodynamic paramenters improves prediction of RNA secondary structure. J. Mol. Biol. 288:911-940[CrossRef][Medline]. |
| 19. |
Mendez, E.,
N. Ruggli,
M. S. Collett, and C. M. Rice.
1998.
Infectious bovine viral diarrhea virus (strain NADL) RNA from stable cDNA clones: a cellular insert determines NS3 production and viral cytopathogenicity.
J. Virol.
72:4737-4745 |
| 20. | Meyers, G., N. Tautz, P. Becher, H.-J. Thiel, and B. M. Kümmerer. 1996. Recovery of cytopathogenic and noncytopathogenic bovine viral diarrhea viruses from cDNA constructs. J. Virol. 70:8606-8613[Abstract]. |
| 21. | Meyers, G., and H.-J. Thiel. 1995. Cytopathogenicity of classical swine fever virus caused by defective interfering particles. J. Virol. 69:3683-3689[Abstract]. |
| 22. | Meyers, G., and H.-J. Thiel. 1996. Molecular characterization of pestiviruses. Adv. Virus Res. 47:53-118[Medline]. |
| 23. | Meyers, G., H.-J. Thiel, and T. Rumenapf. 1996. Classical swine fever virus: recovery of infectious viruses from cDNA constructs and generation of recombinant cytopathogenic defective interfering particles. J. Virol. 70:1588-1595[Abstract]. |
| 24. | Mittelholzer, C., C. Moser, J.-D. Tratschin, and M. A. Hoffman. 1997. Generation of cytopathogenic subgenomic RNA of classical swine fever virus in persistently infected porcine cell culture. Virus Res. 51:125-137[CrossRef][Medline]. |
| 25. |
Moser, C.,
P. Stettler,
J. D. Tratschin, and M. A. Hofmann.
1999.
Cytopathogenic and noncytopathogenic RNA replicons of classical swine fever virus.
J. Virol.
73:7787-7794 |
| 26. | Peek, R., G. J. Pruijn, and W. J. Van Venrooij. 1996. Interaction of the La (SS-B) autoantigen with small ribosomal subunits. Eur. J. Biochem. 236:649-655[Medline]. |
| 27. | Pestova, T. V., and C. U. Hellen. 1999. Internal initiation of translation of bovine viral diarrhea virus RNA. Virology 258:249-256[CrossRef][Medline]. |
| 28. | Pestova, T. V., C. U. Hellen, and I. N. Shatsky. 1996. Canonical eukaryotic initiation factors determine initiation of translation by internal ribosomal entry. Mol. Cell. Biol. 16:6859-6869[Abstract]. |
| 29. |
Pestova, T. V.,
I. N. Shatsky,
S. P. Fletcher,
R. J. Jackson, and C. U. Hellen.
1998.
A prokaryotic-like mode of cytoplasmic eukaryotic ribosome binding to the initiation codon during internal translation initiation of hepatitis C and classical swine fever virus RNAs.
Genes Dev.
12:67-83 |
| 30. | Reynolds, J. E., A. Kaminski, H. J. Kettinen, K. Grace, B. E. Clarke, A. R. Carroll, D. J. Rowlands, and R. J. Jackson. 1995. Unique features of internal initiation of hepatitis C virus RNA translation. EMBO J. 14:6010-6020[Medline]. |
| 31. | Rice, C. M. 1996. Flaviviridae: the viruses and their replication, p. 931-960. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed., vol. 1. Lippincott-Raven Publishers, Philadelphia, Pa. |
| 32. | Rijnbrand, R., P. J. Bredenbeek, T. van der Straaten, L. Whetter, G. Inchauspe, S. Lemon, and W. Spaan. 1995. Almost the entire 5' non-translated region of hepatitis C virus is required for cap-independent translation. FEBS Lett. 365:115-119[CrossRef][Medline]. |
| 33. | Rijnbrand, R., T. van der Straaten, P. A. van Rijn, W. J. Spaan, and P. J. Bredenbeek. 1997. Internal entry of ribosomes is directed by the 5' noncoding region of classical swine fever virus and is dependent on the presence of an RNA pseudoknot upstream of the initiation codon. J. Virol. 71:451-457[Abstract]. |
| 34. |
Rümenapf, T.,
R. Stark,
M. Heimann, and H.-J. Thiel.
1998.
N-terminal protease of pestiviruses: identification of putative catalytic residues by site-directed mutagenesis.
J. Virol.
72:2544-2547 |
| 35. | Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. |
| 36. | Sanderbrand, S. A., N. Tautz, H.-J. Thiel, K. Ochs, E. Beck, and M. Niepmann. 2000. Translation from the internal ribosome entry site of bovine viral dirrhea virus is independent of the interaction with polypyrimidine tract-binding protein. Vet. Microbiol. 77:215-227[CrossRef][Medline]. |
| 37. | Tamura, J. K., P. Warrener, and M. S. Collett. 1993. RNA-stimulated NTPase activity associated with the p80 protein of the pestivirus bovine viral diarrhea virus. Virology 193:1-10[CrossRef][Medline]. |
| 38. | Tautz, N., K. Elbers, D. Stoll, G. Meyers, and H.-J. Thiel. 1997. Serine protease of pestiviruses: determination of cleavage sites. J. Virol. 71:5415-5422[Abstract]. |
| 39. |
Tautz, N.,
T. Harada,
A. Kaiser,
G. Rinck,
S. Behrens, and H. J. Thiel.
1999.
Establishment and characterization of cytopathogenic and noncytopathogenic pestivirus replicons.
J. Virol.
73:9422-9432 |
| 40. |
Tautz, N.,
H.-J. Thiel,
E. J. Dubovi, and G. Meyers.
1994.
Pathogenesis of mucosal disease: a cytopathogenic pestivirus generated by an internal deletion.
J. Virol.
68:3289-3297 |
| 41. | Thiel, H.-J., P. G. W. Plagemann, and V. Moennig. 1996. Pestiviruses, p. 1059-1073. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed., vol. 1. Lippincott-Raven Publishers, Philadelphia, Pa. |
| 42. |
Tsukiyama-Kohara, K.,
N. Iizuka,
M. Kohara, and A. Nomoto.
1992.
Internal ribosome entry site within hepatitis C virus RNA.
J. Virol.
66:1476-1483 |
| 43. |
Wang, C.,
P. Sarnow, and A. Siddiqui.
1993.
Translation of human hepatitis C virus RNA in cultured cells is mediated by an internal ribosome-binding mechanism.
J. Virol.
67:3338-3344 |
| 44. |
Warrener, P.,
J. K. Tamura, and M. S. Collett.
1993.
An RNA-stimulated NTPase activity associated with yellow fever virus NS3 protein expressed in bacteria.
J. Virol.
67:989-996 |
| 45. | Wiskerchen, M., and M. S. Collett. 1991. Pestivirus gene expression: protein p80 of bovine viral diarrhea virus is a proteinase involved in polyprotein processing. Virology 184:341-350[Medline]. |
| 46. | Xu, J., E. Mendez, P. R. Caron, C. Lin, M. A. Murcko, M. S. Collett, and C. M. Rice. 1997. Bovine viral diarrhea virus NS3 serine proteinase: polyprotein cleavage sites, cofactor requirements, and molecular model of an enzyme essential for pestivirus replication. J. Virol. 71:5312-5322[Abstract]. |
| 47. |
Yu, H.,
C. W. Grassmann, and S. E. Behrens.
2000.
A stem-loop motif formed by the immediate 5' terminus of the bovine viral diarrhea virus genome modulates translation as well as replication of the viral genome.
J. Virol.
74:5825-5835 |
| 48. |
Zhong, W.,
L. L. Gutshall, and A. M. Del Vecchio.
1998.
Identification and characterization of an RNA-dependent RNA polymerase activity within the nonstructural protein 5B region of bovine viral diarrhea virus.
J. Virol.
72:9365-9369 |
| 49. | Zuker, M., D. H. Mathews, and D. H. Turner. 1999. Algorithms and thermodynamics for RNA secondary structure prediction: a practical guide. Kluwer Academic Publishers, Dordrecht, The Netherlands. |
Journal of Virology, May 2001, p. 4226-4238, Vol. 75, No. 9
0022-538X/01/$04.00+0 DOI: 10.1128/JVI.75.9.4226-4238.2001
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