Department of Molecular Genetics and Microbiology, School of Medicine, State University of New York at Stony Brook, Stony Brook, NY 11794, USA1
Biochemistry and Molecular Biology, Chiron Corporation, Emeryville, CA 94608, USA2
Author for correspondence: Eckard Wimmer. Fax +1 631 632 8891. e-mail ewimmer{at}ms.cc.sunysb.edu
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Abstract |
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Introduction |
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The enterovirus and rhinovirus genomes are about 7500 nucleotides long, with a small viral protein (VPg) and a poly(A) tail present at their 5' and 3' termini, respectively (Kitamura et al., 1980 , 1981
; Lee et al., 1977
; Skern et al., 1985
). Both enterovirus and rhinovirus genomes encode a single large polyprotein from which the viral structural proteins, expressed as precursor P1, and non-structural proteins, as expressed as P2 and P3, are derived by proteolytic processing (Fig. 1b
). The processing steps are catalysed by the virus-encoded proteinases 2Apro, 3Cpro and 3CDpro. The 2Apro proteinases are encoded immediately downstream of the P1 precursor in enterovirus and rhinovirus genomes. This proteinase cleaves the P1P2 junction in cis and cellular proteins in trans. The cis-cleavage activity of the enterovirus and rhinovirus 2Apro proteinases releases the P1 precursor from the non-structural P2P3 precursors (Sommergruber et al., 1989
; Toyoda et al., 1986
). The trans-cleavage activity of enterovirus and rhinovirus 2Apro processes cellular factors, including eukaryotic initiation factor eIF-4G (eIF-4
or p220) (Kräusslich et al., 1987
; Lamphear et al., 1993
), TATA-binding protein (Yalamanchili et al., 1997
), poly(A)-binding protein (PABP) (Joachims et al., 1999
; Kerekatte et al., 1999
), dystrophin (Badorff et al., 1999
) and the viral protein 3CDpro (Lee & Wimmer, 1988
). With the exception of eIF-4G, the effects of the 2Apro trans-cleavage activity on cellular proteins are not clear. Cleavage of eIF-4G, and possible also of PABP, contributes to the shut-off of host cell protein synthesis (Joachims et al., 1999
; Kräusslich et al., 1987
). Translation is thus switched from cap-dependent cellular translation to cap-independent viral translation. Shut-off of host cell protein synthesis can also result in a process of programmed cell death (Barco et al., 2000
; Goldstaub et al., 2000
). The precise function of 2Apro in the cleavage of eIF-4G is presently debated. Proteinase 2Apro is definitely responsible for the direct cleavage of cellular proteins (Haghighat et al., 1996
; Lamphear et al., 1993
; Liebig et al., 1993
), but evidence for activation of cellular activities has also been presented in eIF-4G processing (Bovee et al., 1998a
, b
). The cleavage of dystrophin of mouse heart muscle cells by coxsackievirus B3 2Apro has been suggested to be the mechanism of dilated cardiomyopathy (Wessely et al., 1998
). The 2Apro cleavage products of 3CDpro (3C' and 3D') are not essential for poliovirus replication (Lee & Wimmer, 1988
).
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Genetic data suggest that 2Apro is an important component for poliovirus RNA replication, but the function remains elusive (Ansardi et al., 1995 ; Molla et al., 1992
, 1993b
; ONeill & Racaniello, 1989
; Yu et al., 1995
). Although not endowed with strong hydrophobic sequences, poliovirus 2Apro was found in the detergent-insoluble membranes (Martin-Belmonte et al., 2000
). Not surprisingly, the 2A proteins of hepatitis A virus and Theilers murine encephalomyelitis virus do not seem to be required for virus RNA replication (Harmon et al., 1995
; Michiels et al., 1997
), since these viral polypeptides bear no similarity to the entero- and rhinovirus 2Apro enzymes (Gromeier et al., 1999
).
In our previous study, we have demonstrated that mutations at the P5 position of coxsackievirus B4 (CBV4) 2Apro promoted viral RNA replication of a chimeric poliovirus in which the cognate poliovirus 2Apro sequence was exchanged for that of CBV4. Chimeric poliovirus genomes with an HRV2 2Apro-encoding sequence did not produce viable virus, but showed both a low level of viral RNA replication (detected by RTPCR) and minor alternations in processing of P2 proteins (Lu et al., 1995b ). Amino acid alignments show that the C terminus of the HRV2 2Apro lacks four amino acids compared with the C terminus of 2Apro from poliovirus type 1 Mahoney [PV1(M)] (Fig. 1a
). These four amino acids (EAME) correspond to an acidic domain preserved among enterovirus 2Apro polypeptides. In this paper, we have used site-directed mutagenesis to show that the conserved C terminus of PV1(M) 2Apro plays an important role in viral RNA replication.
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Methods |
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Oligonucleotides.
The following oligonucleotide primers were used in this study: 5101 (5' CGGAGACGCCAAAAA 3'), 5120 (5' CTGAGCTCCAATTTGGACTTTCCGCC 3'), L2 (5' CCAAGGAGCTCACCAC 3'), 17 (5' GAGGCCTTGTTCGTAGGCATACAAGTC 3'), 25 (5' GAGGCCCTGCTCCATTGCCTCTTCTTCGTAGGCATACAAGTC 3'), 4578 (5' GCGGAGCTCACTACAGCTGGCCCC 3') and 5040 (5' GGAGGCCTTGTTCCATGGCTTCTTCTTCAGCACAAT 3').
DNA manipulations.
Escherichia coli strain DH5 was used for plasmid transformation and propagation. DNA cloning was accomplished by standard procedures (Sambrook et al., 1989
). Cloning enzymes and reagents were purchased from New England Biolabs or Boehringer Mannheim. pT7PVM(S+E-) is a full-length poliovirus cDNA clone that contains two engineered restriction sites (EcoRI and SacI) downstream of an authentic AUG codon (Mueller & Wimmer, 1998
). pT7S/2A/S is a full-length poliovirus cDNA clone with a SacI site at the junction of the P1- and 2A-encoding sequences (Lu et al., 1995b
). pT7PVM(S+E-) and pT7S/2A/S were digested by NheI and BglI and ligated to yield the cDNA plasmid pT7S+E-S/2A/S. PCR-amplified luciferase-encoding sequences (primers 5101 and 5120) were used to replace the P1 region between the EcoRI and SacI sites of pT7S+E-S/2A/S to generate a PV1(M) replicon plasmid PVM/Luc. The different 2Apro-encoding sequences were amplified by PCR and cloned into the SacI and StuI sites of the PVM/Luc plasmid. New chimeric poliovirus replicon clones contained wild-type HRV2 2Apro sequences (PVM/Luc R2A), the truncated C-terminal five amino acids (P2P6) of PV1(M) 2Apro (PVM/Luc C-5) (primers L2 and 17) and HRV2 2Apro with four amino acids (P2P5) from the C terminus of PV1(M) 2Apro (PVM/Luc R2A C+4) (primers 4578 and 5040). To determine whether the C-terminal sequences of 2Apro act at the level of RNA or protein, mutations (P1P4) were made at every wobble position, generating silent mutations (PVM/Luc Cm4) (primers L2 and 25). At the same time, the various modified 2Apro sequences were introduced into full-length pT7S/2A/S cDNA clones. The new chimeric PV1(M) full-length clones were named PVM Cm4, PVM C-5 and PVM R2A C+4. PVM R2A is identical to PV/HRV2-2A (Lu et al., 1995b
). The details of the C-terminal modifications are shown in Fig. 1(b)
.
In vitro transcription, translation and Western blotting.
In order to produce the RNA transcripts in vitro, 0·7 µg of each full-length and replicon cDNA plasmid was linearized by PvuI downstream from the viral genome (Alexander et al., 1994 ; Lu et al., 1995a
, b
). RNA transcripts were synthesized from the linear template DNA by use of T7 RNA polymerase in 100 µl of an in vitro transcription reaction mixture. RNA transcripts were purified by phenolchloroform extraction and ethanol precipitation. For each RNA transcript, the optimal RNA concentration was determined for in vitro translation in HeLa cell extracts as described by Molla et al. (1991)
. Translation reactions were carried out at 34 °C for 7 h in the presence of 10 µCi of [35S]-translabel (Amersham). SDS12·5% polyacrylamide gels were used to analyse the translation products (Laemmli, 1970
). The intensity of the VP3 band of each poliovirus full-length RNA translation reaction was measured by using the Un-Scan It program (Silk Scientific Company). Translation efficiency was calculated as described previously (Lu et al., 1995b
). Briefly, the translation efficiency of PVM R2A RNA was taken as 100%. The translation efficiency of each chimeric RNA was calculated from the relative intensity of the VP3 band compared with the intensity of the VP3 band from PVM R2A RNA.
Western blotting was used to detect degradation products of eIF-4G. Briefly, in vitro translation reactions were carried out in 62·5 µl of total translation reactions for each full-length RNA transcript at 30 °C for 24 h. TCA precipitation (8%) was used to reduce the sample volume. The samples were analysed on 7·5% SDSPAGE and transferred overnight at 4 °C to a nitrocellulose membrane (Schleicher & Schuell). The nitrocellulose membrane was incubated at room temperature for 2 h with a rabbit anti-eIF-4G primary antibody (Aldabe et al., 1995 ) and then incubated at room temperature for an additional 2 h with HRP-conjugated goat anti-rabbit antibodies (Cappel) as secondary antibodies. Degradation products of eIF-4G were detected by ECL (Amersham) followed by exposure of the membrane to Kodak X-ray film for 5 min.
RNA transfections.
To perform the RNA transfection, HeLa R19 cells cultured on a 35 mm plate were incubated with 510 µg of RNA transcripts in the presence of 0·5 mg/ml DEAEdextran in HeBSS buffer (42 mM HEPES, 270 mM NaCl, 9·6 mM KCl and 1·4 mM Na2HPO4) at room temperature for 30 min. The transfection mixtures were removed and the cells were cultured in 2 ml DMEM2% BCS at 37 °C (Sambrook et al., 1989 ). HeLa cell monolayers were harvested at different time-points.
Trans-rescue assay.
The trans-rescue assay was performed as described previously (Hambidge & Sarnow, 1992 ). Briefly, the DNA transfection was performed with calcium phosphate by incubating 1 µg of the PV1(M) replicon cDNA plasmids and 10 µg of the pBS, pBS E2A and pBS E2A(CH) cDNA plasmids on OST7-1 monolayers. Glycerol shock was carried out at 6 h after addition of the DNA/calcium phosphate precipitate. Transfected OST7-1 cells were incubated at 37 °C with 5% CO2 for another 12 h (Ausubel et al., 1994
). The harvested OST7-1 cells were resuspended in PBS for luciferase assays as described below.
Encapsidation assay.
Encapsidation assays were performed according to Ansardi et al. (1991 , 1993
). The PV1(M) replicon RNA transcripts were transfected into HeLa cell monolayers 2 h after VV-P1 infection. HeLa cell monolayers were cultured in 1·5 ml of DMEM2% BCS at 37 °C for 24 h. HeLa cell lysates were obtained by freezethawing three times. Aliquots of 250 µl of the cell lysates were inoculated onto another set of fresh HeLa cell monolayers, which were harvested at 0, 2, 4, 6, 8 and 10 h post-infection. The cell lysates were analysed for luciferase activity.
Luciferase assay.
After transfections of RNA or DNA containing the luciferase gene, HeLa cell or mouse cell monolayers were harvested by washing three times with PBS and resuspending the cell pellet in 100 µl PBS (Ausubel et al., 1994 ). The cells were lysed immediately by freezethawing three times. Twenty µl of cell lysate was examined by adding 100 µl luciferin to measure luciferase activity in a luminometer (Promega). The protein concentration (125 µg) of each cell lysate was determined by a Micro BCA protein assay (Pierce) as an internal control to normalize the luciferase activities (Ventoso & Carrasco, 1995
).
Plaque assays.
Plaque assays on HeLa cell monolayers were performed as described previously (Lu et al., 1995b ). The virus was diluted in PBS and placed on the cells. The mixture was incubated for 30 min at room temperature to allow the virus to absorb to the cells and then 3 ml of 1x DMEM plus 10% calf serum (Gibco-BRL) plus 1% agar was added to each plate. After incubation for 2 days, the agar overlays were removed and the cells were stained with crystal violet.
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Results |
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Translation efficiencies and proteolytic activities of viral RNAs with modifications in the 2Apro C-terminal domain
To investigate the pronounced effect of the C-terminal domain of 2Apro on virus proliferation, we have analysed the modified viral genomes by several methods. Firstly, we determined the efficiency with which the RNA could direct faithful protein synthesis. Translation of the RNAs was performed in HeLa cell extracts (Molla et al., 1991 ). Chimeric PV1(M) full-length RNA transcripts with modified 2Apro C termini translated nearly as well as those of wild-type 2Apro (Fig. 2a
; lanes 48). This was determined by measuring the VP3 intensity and calculating the translation efficiency for each translation reaction as described in Methods. The translation efficiency of each chimeric PV1(M) RNA is given at the bottom of Fig. 2(a)
. With PVM Cm4, neither the relative mobility of 2Apro nor the translation efficiency was altered, as expected (Fig. 2a
; lanes 4 and 5). PVM C-5 RNA transcripts, in which five amino acids had been deleted, translated as well as PV1(M) and PVM Cm4 RNA transcripts (Fig. 2a
; compare lanes 4 and 5 with lane 6). The relative mobility of 2Apro in PVM C-5 increased, however (lane 6). On the other hand, addition of four amino acids to HR2 2Apro (PVM R2A C+4) decreased the relative mobility of HRV2 2Apro and the protein migrated to the same position as PV1(M) 2Apro (lane 7). The translation efficiency of PVM R2A C+4, however, was reduced slightly (Fig. 2a
, lane 4 and 7). The cleavage patterns seen in lanes 6, 7 and 8 clearly reveal a few aberrant cleavage products in addition to all the major viral polypeptides.
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The endogenous cellular protein eIF-4G was used to examine the trans-cleavage activity of PV1(M) and HRV2 2Apro proteinases with modified C termini by Western blotting. Intact eIF-4G protein is shown in the no-RNA control (Fig. 2c; lane 1). Completely degraded eIF-4G products were detected in all translation reactions (Fig. 2c
; lanes 26). No differences in eIF-4G cleavage were observed between the wild-type 2Apro (Fig. 2c
; lanes 2 and 6) and modified 2Apro (Fig. 2c
; lanes 35). Thus, the C-terminal modifications did not affect the proteolytic activity in trans of PV1(M) and HRV2 2Apro proteinases.
The function of the C-terminal domain of PV1(M) 2Apro in viral RNA replication
It has been reported that the addition of a foreign gene (Alexander et al., 1994 ) or the replacement of the poliovirus P1 region by a reporter gene does not affect poliovirus replication, including viral protein processing, RNA synthesis or encapsidation in trans (Porter et al., 1998
; for references see Mueller & Wimmer, 2000
). Our previous results showed that a chimeric PV1(M) genome with HRV2 2Apro did not produce virus but suggested very low levels of viral RNA replication (Lu et al., 1995b
). Since the pattern of protein synthesis and proteolysis in vitro showed production of all proteins involved in RNA synthesis, we decided to investigate whether the 2Apro C termini have a function in RNA replication. To monitor replication, we constructed PV1(M) replicon genomes containing the luciferase gene. After transfection into HeLa cells, the luciferase activity was measured. The transfected HeLa cell monolayers were incubated at 37 °C and cells were lysed at 0, 4, 8, 12 and 24 h post-transfection. Luciferase activity generated by PVM/Luc and PVM/Luc Cm4 RNA transcripts was detected at 4 h and it reached a peak at 8 h post-transfection (Fig. 3a
; open squares). At this time-point, the luciferase activity produced by PVM/Luc R2A was nearly 1000-fold lower than that of PVM/Luc, while a detectable signal emerged only 12 h post-transfection (closed circles). Remarkably, addition of the four amino acids to the C terminus of HRV2 2Apro in PVM/Luc R2A C+4 genomes increased the expression and led to a signal at 8 h post-transfection that was about 100-fold greater than that of PVM/Luc R2A (open circles) (Fig. 3a
) and only 10-fold lower than that of PVM/Luc. The luciferase activity of PVM R2A C+4 reached its peak at 12 h post-transfection. No luciferase activity above background could be detected with PVM/Luc C-5 RNA.
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Trans-rescue of the C-terminally modified 2Apro with wild-type and mutated poliovirus 2Apro
In order to test whether the C-terminal functions of 2Apro could be rescued in trans, we pursued a trans-rescue assay in a mouse fibroblast cell line, OST7-1, that expresses phage T7 RNA polymerase in the cytoplasm. T7 RNA polymerase can be used to transcribe RNA from transfected cDNA plasmids containing the T7 promoter. Since transcription in all of our cDNA plasmids is driven by the T7 promoter (van der Werf et al., 1986 ), we were able to co-transfect PV1(M) replicon cDNA plasmids, together with expression plasmids for PV1(M) 2Apro cDNA [pBS E2A or pBS E2A(CH)], into OST7-1 cells and assay for complementation by monitoring luciferase activity. Results of such co-transfection experiments are shown in Fig. 4
. Transfection with vectors containing no luciferase gene gave background signals (Fig. 4
; group A, bars 25). Co-transfection of different poliovirus-expression vectors is presented in groups as follows: (B) wild-type PVM/Luc, (C) PVM/Luc Cm4; (D) PVM/Luc C-5; (E) PVM R2A C+4 and (F) PVM/Luc R2A, involving either pBS or 2A-expressing plasmids, as indicated. If guanidineHCl was omitted at the beginning of co-transfection, all plasmids, with the exception of PVM/Luc C-5 (Fig. 4
; group D, bar 14), yielded strong luciferase signals (bars 6, 10, 18 and 22), which can be assumed to be the result of mRNA production by transcription and replication. This is supported by the observation that guanidineHCl reduced the signal obtained in these cells to the level of PVM/Luc C-5 (compare bars 7, 11, 19 and 23 with bar 15). Co-transfection with a plasmid expressing 2Apro under the control of the EMCV IRES stimulated the luciferase signal (see bars 8, 12, 16, 20 and 24), although the increase was barely detectable in group F (bar 24). However, the 12·7-fold increase (bar 16) is highly significant and required expression of active proteinase, since expression of inactive proteinase had no effect on the luciferase signal (bars 9, 13, 17, 21 and 25).
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Discussion |
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In our previous studies, we showed that 2Apro of CBV4, another enterovirus, could replace the poliovirus 2Apro in a chimera. However, mutations in the C terminus of CBV4 2Apro were necessary to yield a chimera with wild-type replication properties (Lu et al., 1995b ). These mutations all mapped to precisely the region that is missing in HRV2 2Apro. Thus, we both modified this region in poliovirus 2Apro and added four amino acids to HRV2 2Apro to create an enterovirus-like 2Apro. In all constructs, the P1P2 junction of the PV1(M) polyprotein is LtTY*GfGh, where capital letters represent residues conserved among polioviruses (Hellen et al., 1992
); ITTA*GPSD is the corresponding sequence in HRV2 (Skern et al., 1991
). To facilitate 3CDpro cleavage activity at the 2A2B junction, the P4 position for each C-terminal modification was alanine, a residue greatly preferred by poliovirus 3CDpro cleavage activity (Fig. 1b
) (Lawson & Semler, 1990
).
To study the C-terminal functions of PV1(M) and HRV2 2Apro in terms of their proteolytic activities, the RNA transcripts were translated in HeLa cell extracts. Even when five amino acids (P2P6) were deleted at the C-terminal domain of PV1(M) 2Apro (PVM C-5), neither translation efficiency nor the cis- and trans-cleavage activities was affected significantly (Fig. 2a, lanes 4 and 6; Fig. 2c
, lanes 2 and 4). Deletion of a further nine amino acids at the C terminus of poliovirus 2Apro abolished the cis-cleavage activity (Toyoda et al., 1986
). Insertions at the N and C termini also abolished cis-cleavage activity of PV1(M) 2Apro (Bernstein et al., 1986
; Kräusslich et al., 1987
). On the other hand, a C-terminal deletion of up to six amino acids of HRV2 2Apro did not interfere with its cis-cleavage activity, whereas a deletion of up to 10 amino acids inactivated the enzyme (Sommergruber et al., 1989
). Translation with chimeric PVM R2A C+4 and PVM R2A genomes showed that all expected proteins were produced by proteolytic processing (Fig. 2a
; lanes 7 and 8). Importantly, none of the 2A modifications at the C terminus impaired the enzymes ability to cleave eIF-4G (Fig. 2c
; lanes 5 and 6).
Whereas the C-terminal deletions caused little if any loss of cleavage activity for either PV1(M) or HRV2 2Apro, severe replication phenotypes were observed. We conclude that the C-terminal domain up to amino acid 6 is not critical for proteolytic activities of poliovirus 2Apro, but this conclusion is based solely on in vitro translation assays. A correlation between the structure and the function of poliovirus 2Apro remains to be done.
The involvement of PV1(M) 2Apro in viral RNA replication was suggested by Molla et al. (1993b ) from experiments using dicistronic poliovirus genomes. While the insertion of an EMCV IRES at the P1P2 junction of the poliovirus genome did not interfere with either proteolytic processing or genome replication, deletion of 2Apro in these constructs and even mutation of C109A abolished RNA synthesis (Molla et al., 1992
, 1993b
). Yu and colleagues (Yu et al., 1995
; Yu & Lloyd, 1991
) have come to the same conclusion, based on mutations introduced into the catalytic triad or other conserved residues of the 2Apro molecule. So far, two features of PV1(M) 2Apro seem to be important for this protein to promote RNA replication: the identity of C109 of the catalytic triad and the presence of four amino acid residues (P2P5) at the C terminus. Whether the importance of both of these features relates to a specific structure of 2Apro remains to be seen. It is possible that a cluster of negatively charged amino acids involving the sequence EAME may play a role in poliovirus RNA replication. This would explain why the addition of the four amino acids EAME to HRV2 2Apro greatly improved replication of the chimeric replicon PVM/Luc R2A C+4 (Fig. 3a
; open circles). A poliovirus genomic chimera in which the cognate 2Apro was replaced with R2A C+4 did not yield viruses, however (data not shown). These observations led originally to our speculation that the nucleotide sequence encoding 2Apro may be involved in encapsidation. A change of four nucleotides of the EAME-encoding nucleotide sequence at the C terminus (2A Cm4) did not yield a replication phenotype, however. The high yield at which PVM/Luc R2A C+4 was encapsidated in trans (Fig. 5
, open circles) must, therefore, relate to the ability of PVM/Luc R2A C+4 to replicate, rather than to a specific encapsidation signal. This leaves unexplained the surprising observation that the R2A C+4 RNA does not form virions. Experiments to find escape mutants have failed, but they have not yet involved long-term, blind passages.
Encapsidation signals residing in virus genomes have been identified for several RNA viruses, for example retroviruses (Clever et al., 1995 ; Mansky et al., 1995
) and a togavirus (Weiss et al., 1989
). Encapsidation of poliovirus is specific in that the virus particle only contains VPg-linked, positive-sense poliovirus RNA. Thus, the encapsidation process discriminates against virus mRNA, lacking VPg, and minus-sense RNA. An encapsidation signal in poliovirus plus-stranded RNA has not yet been discovered, however. Numerous studies have led to the exclusion of possible signals, such as the IRES element and regions in the coding sequences of P1 and VPg, or VPg itself (Barclay et al., 1998
; Gromeier et al., 1996
; Lu & Wimmer, 1996
; Porter et al., 1998
; Reuer et al., 1990
). Studies using the cell-free, de novo synthesis of poliovirus (Molla et al., 1991
) or genetic analyses of replicons (Nugent et al., 1999
) have suggested that genome replication is necessary for encapsidation. The data presented here support these previous conclusions. The mechanism by which the plus-stranded viral RNA is selected for encapsidation remains elusive, however. Another less-likely possibility is that an intact, virus-specific 2Apro molecule is involved directly in virus particle formation, since non-structural proteins have been discovered in virus particles of foot-and-mouth disease virus and poliovirus (Newman et al., 1994
).
Co-transfection of plasmids expressing luciferase-containing replicons with plasmids expressing poliovirus 2Apro resulted in all cases in an increased signal of the reporter gene products (Fig. 4). Such an effect on translation efficiency has been observed before (Hambidge & Sarnow, 1992
) and may be due to a specific but as yet undefined interaction of the proteinase with the poliovirus IRES element (Macadam et al., 1994
; Rowe et al., 2000
) combined with a more rapid degradation of eIF-4G. In agreement with this, co-expression of a mutant enzyme (2Apro CH) had no effect on the luciferase signal. However, the increase in the luciferase signal of the replication-incompetent replicon PVM/Luc C-5 (Fig. 4
; bar 16) may reflect trans-activation of RNA replication, since the IRES sequence in this replicon is identical to that in the others.
The 2Apro enzyme of poliovirus has multiple functions, for which stringent structural parameters may be essential. The integrity of the catalytic triad (particularly of C109) appears to play an important role in all functions. We have identified a new structural determinant for genome replication, the C-terminal five amino acids.
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Acknowledgments |
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Received 3 August 2000;
accepted 19 October 2000.