1 Department of Molecular Microbiology and Immunology, Saint Louis University School of Medicine, 1402 South Grand Avenue, St Louis, MO 63104, USA
2 Center for Macromolecular Crystallography, University of Alabama at Birmingham, 79-THT, MCLM-244, 1918 University Boulevard, Birmingham, AL 35294-0005, USA
Correspondence
Thomas J. Chambers
thomas_chambers2{at}merck.com
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ABSTRACT |
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INTRODUCTION |
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In previous studies, it was established that NS3 cleavage activity is necessary for correct processing of the viral polyprotein and for virus replication (Chambers et al., 1990b; Wengler et al., 1991
). NS3 and NS2B form a stable complex that cleaves the polyprotein substrate in cis and in trans (Arias et al., 1993
; Chambers et al., 1993
; Falgout et al., 1993
), although the factors governing the sequence of cleavages needed for assembly of RNA replication complexes remain poorly understood. The molecular basis for NS2BNS3 complex formation involves both a conserved central region within NS2B, and the amino-terminal region of NS3 (Chambers et al., 1993
; Droll et al., 2000
; Falgout et al., 1993
). Within the conserved region, there is a potential peptide cofactor analogous to that of the NS4A protein that complexes with the NS3 protease of hepatitis C virus (Brinkworth et al., 1999
; Butkiewicz et al., 1996
; Lin et al., 1995
). However, for YFV, charged amino acids are involved in the complex formation. In previous studies, we analysed a series of charged-to-alanine mutations within the NS2BNS3181 polyprotein for effects on processing of the viral polyprotein (Droll et al., 2000
). Because these mutations caused a range of effects on cleavage efficiency, it was of interest to determine what effects impairment of cleavage activity would have on viral infectivity. Identification of mutations that are deleterious for virus replication but do not interfere with cleavage activity could suggest novel functions of either NS2B or NS3 based on proteinprotein interactions with other viral or host proteins.
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METHODS |
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Plasmid constructions.
Mutations were originally created in pET/BS-NS2BNS3181 as described previously using a QuikChange Site-Directed Mutagenesis protocol (Stratagene) (Droll et al., 2000). pET/BS-NS2BNS3181 (formerly named pET/BS-NS2B3·1) is a phagemid, derived originally by engineering an FspI/ScaI restriction fragment from pBluescriptII SK(+) (Stratagene) containing the f1 origin, into pET8C-NS2B3·1, as described previously (Chambers et al., 1990b
). The transcription vector pET8C (Studier et al., 1990
) contains a promoter for T7 RNA polymerase, followed by a unique NcoI site with an ATG in an appropriate context for eukaryotic expression. pET8C-NS2B3·1 was originally created by inserting a PCR-amplified fragment obtained from YFM5·2 DNA (Rice et al., 1989
), encompassing the NS2BNS3181 region together with a 5' NcoI site and a 3' BamHI site adjacent to a translation termination codon, into pET8C using NcoI and BglII restriction sites, as described (Chambers et al., 1990b
).
For transient expression experiments of mutant YF non-structural polyproteins in SW-13 and BHK-21 cells, mutations in pET/BS-NS2BNS3181 were subcloned into pET/BS-sig2A5356 (Chambers et al., 1991). SacI and PvuII restriction sites were used to introduce the mutations from pET/BS-NS2BNS3181 into pET/BS-sig2A5356. YF5·2iv templates needed for the generation of infectious YF RNA transcripts containing the mutations required engineering the individual NS2B or NS3 mutations into pYFM5·2, which is part of a two-plasmid system used for production of in vitro-ligated full-length viral transcription templates (Rice et al., 1989
), as described below. The mutations were exchanged from pET/BS-sig2A5356 into pYFM5·2 using AvrII and NgoMI restriction sites. Presence of the desired mutations in pYFM5·2 was confirmed by nucleotide sequencing.
Cell-free translation.
Protease cleavage activity at the 2B/3 cleavage site was analysed by cell-free translation by using the TNT Coupled Reticulocyte Lysate system (Promega). Reactions were run as recommended by the manufacturer except reaction volumes were scaled down to half the volume (25 instead of 50 µl). Reactions were programmed with 1 µg unlinearized plasmid DNA (parental pET/BS-NS2BNS3181 or various mutant derivatives). Translation products were labelled by the addition of 1 µCi (37 kBq) of [35S]methionine (0·4 mCi µl1) per reaction, and run for 20, 45 and 90 min. For reactions run in the presence of canine pancreatic microsomal membranes (Y4041; Promega), 1·5 µl stock membrane preparation was added to each reaction, which in control experiments was sufficient to glycosylate the control protein and to cleave the signal sequence from the control protein. Translation products were immunoprecipitated by using conditions previously described (Droll et al., 2000), and analysed on SDS-PAGE with imaging by fluorography.
Transient expression of sig2A5356 polyproteins.
Transfection of the pET/BS-sig2A5356 plasmid for expression of the YF non-structural polyprotein containing the 2A/2B, 2B/3, 3/4A, 4A/2K, 2K/4B and 4B/5 cleavage sites was done in SW-13 and BHK-21 cells essentially as described previously (Droll et al., 2000), except for the use of lipofectamine. Cells were preinfected with vaccinia virus vTF7-3 (10 p.f.u. per cell), which encodes the bacteriophage T7 RNA polymerase under the control of an early vaccinia promoter, and then transfected with plasmid DNA to drive RNA synthesis from the T7 promoter encoded upstream of the YF non-structural protein genes. Transfection reactions were done in six-well costars by the addition of a mixture of 4 µl Lipofectamine, 6 µl Plus reagent (Invitrogen) and 1 µg caesium-banded plasmid DNA in a final volume of 400 µl
-MEM per well. Transfection was continued for 2·5 h, followed by addition of [35S]methionine and labelling for an interval of 4·55 h. Cells were harvested by the addition of 0·5 ml SDS lysis buffer (0·5 % SDS, 10 mM Tris/HCl pH 7·5, 150 mM NaCl, 1 mM EDTA) at 25 °C, sheared by passage through a 26-gauge needle and centrifuged in an Eppendorf centrifuge for 10 min to remove insoluble material. SDS lysates were diluted to 1x Triton solution (1 % Triton X-100, 10 mM Tris/HCl pH 7·5, 150 mM NaCl, 1 mg BSA ml1), and chilled at 4 °C for 15 min. Virus-specific proteins were immunoprecipitated with specific rabbit polyclonal antisera to the YF NS2B, NS3 or NS4B proteins as described previously (Chambers et al., 1990a
) and immunoprecipitates were analysed by SDS-PAGE on 1013 % SDS gels as previously described (Chambers et al., 1990a
; Droll et al., 2000
).
Transcription and transfection.
A two-plasmid system for construction of YF5·2iv virus templates was used as previously described (Rice et al., 1989). The templates were assembled by ligation of the appropriate restriction fragments, and full-length RNA transcripts were synthesized by using SP6 RNA polymerase in the presence of 5' cap analogue (New England Biolabs). Transfections were done by incubating Vero cells at 25 °C for 10 min in the presence of a mixture of 100300 ng RNA transcripts and 20 µl lipofectin (Gibco-BRL) in PBS in a reaction volume of 500 µl. Transfected cell cultures were incubated at either 32 or 37 °C and viruses were harvested at the time of onset of cytopathic effects, usually at 5 to 7 days after transfection. Virus yields were determined by plaque assay on SW-13 cells and plaque sizes were determined as the mean diameters of 10 well-isolated plaques.
Plaque purification.
Mutant viruses recovered from RNA transfections were plaque-purified three times in SW-13 cells with amplification on BHK-21 cells. Concentrated virus stocks were prepared for some of the mutants by precipitation with PEG-8000. The virus solution was adjusted to a concentration of 10 % PEG-8000 in TNE (120 mM NaCl, 12 mM Tris/HCl pH 8·0, 1 mM EDTA), the material was placed on ice for 1 h, and the precipitated virus was recovered by centrifugation in a Sorvall centrifuge using a GSA rotor at 5000 r.p.m. for 30 min at 4 °C. The pellet was gently washed twice with TNE, and finally resuspended in alpha-MEM plus 20 % fetal calf serum, at 1 : 100 of the original volume of the virus solution. Virus was aliquotted and stored at 70 °C until use.
Growth curve analysis.
Growth curve experiments were done by infecting SW-13 or C6/36 cell monolayers at an m.o.i. ranging from 1 to 5 (m.o.i. of 5 were used unless limited by titre of the virus). Parental and mutant growth curve infections were always in parallel using identical m.o.i values. Media were harvested at approximately 1224 h intervals and replaced with fresh media (alpha-MEM plus 3 % FBS). Samples were assayed in triplicate by plaque assay on SW-13 cells.
Isolation and sequencing of revertant viruses.
Plaque-revertant viruses were isolated during plaque purification of the mutant viruses, and subjected to at least one round of plaque purification in duplicate for each revertant undergoing characterization. RNA was prepared from the plaque isolates by extraction of infected cell monolayers with Trizol (Gibco-BRL). One microgram of RNA was reverse-transcribed using Superscript II (Gibco-BRL), in the presence of an antisense oligonucleotide primer corresponding to YF nt 53005320. cDNA was amplified by PCR using the same 3' primer and a 5' primer (nt 41414160), encompassing the NS2BNS3181 region, in the presence of Taq DNA polymerase (Gibco-BRL). PCR products were purified with Wizard PCR preps kits (Promega), and sequenced using BigDye chain terminator reactions on a Becton Dickinson ABI DNA sequencer.
Construction of plasmids containing reversion mutations.
Mutations identified by sequencing of PCR products from plaque-purified revertant viruses were subcloned directly into pET/BS-NS2BNS3181 using available restriction sites. Where this was not possible, PCR products were reamplified using the 3' primer YF 5300, and a 5' primer incorporating an XbaI site adjacent to the 5' terminus of the NS2B region, and cloning the resulting PCR product into pET/BS-NS2BNS3181 using the XbaI and HpaI restriction sites. In some cases, the PCR products were initially subcloned into the TOPO-TA vector (Invitrogen), before cloning into pET/BS-NS2BNS3181.
Molecular modelling.
A homology model for the YFV NS3 protease was derived on the basis of the reported crystal structure of the dengue-2 protease (PDB accession no. 1bef; GenBank accession no. M14969), using the template and coordinates provided by the Swiss-modeller program. Figs were drawn using graphic programs supplied by the modelling server.
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RESULTS |
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Fig. 1 illustrates the mutations which were engineered into the YF5·2iv molecular clone. Table 1
summarizes the data on recovery of viruses, their relative plaque sizes formed at 37 °C on SW-13 cells, and the corresponding level of 2B/3 cleavage activity based on cell-free assay (Droll et al., 2000
). The mutations had variable effects on recovery of infectious virus and plaque size. Thirteen mutants had a parental phenotype (>90 % of parental size). Seventeen mutants had a reduced plaque-phenotype (5090 % of parental size). Eight mutants had a small plaque-phenotype (<50 % of parental). Eight mutants did not form plaques. Four mutations were not tested for recovery of virus. Virus titres after RNA transfection indicated no severe defect in replication efficiency for those mutants detectable by plaque assay, based on recovery of more than 104 p.f.u. virus ml1. Furthermore, transfection at 32 versus 37 °C yielded no evidence that any mutant displayed a temperature-sensitive phenotype. In these experiments, virus yields from the transfection harvest for the parental YF5·2iv were in the range of 5x106 to 1x107 p.f.u. ml1. Mutant viruses selected for further study by growth curve analysis, polyprotein cleavage assays and revertant characterization are indicated in the table.
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Growth curve analysis
To determine if reduced plaque-size reflected impaired replication efficiency as measured by virus production in cell culture, a number of the small plaque-mutant viruses were selected for growth curve analysis. Mutants that exhibited a range of cleavage efficiency at the 2B/3 cleavage site were studied (2·5, 3·7, 3·12 and 3·22). However, not all mutants could be studied in this way because either a high rate of plaque reversion precluded preparation of some plaque-purified virus stocks (2·3 and 2·18) or execution of the growth curve was complicated by appearance of plaque revertants (2·4). Results of the growth curve studies are shown in Fig. 2(a)(d). Studies were done in SW-13 cells at 37 and 32 °C to screen for temperature sensitivity, and for some mutants also in C6/36 cells at 30 °C, to extend the range for temperature-sensitive screening, and test for any evidence of host-restriction of virus replication.
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Fig. 2(b) shows results for mutation 3·12, which caused a mild decrease in 2B/3 cleavage (88 %), and caused a small plaque-size (41 % of parental virus). Its growth was characterized by reduced virus production at 37 °C (panel i) (1 log lower peak-titre than the parent virus), but a less severe defect at 32 °C (panel ii) (0·3 log lower peak-titre), in SW-13 cells. Growth in C6/36 cells at 30 °C (panel iii) was similar to parental virus, suggesting increased stability of the mutant virus at this temperature.
Fig. 2(c) shows the results for mutation 3·15, which caused no defect in cleavage at the 2B/3 site (91·7 %), and caused a small plaque-size (33 % of parental size). It exhibited a small reduction in virus production at both 37 and 32 °C (panels i and ii, respectively), with decreases of 0·4 and 0·3 logs of virus, respectively, on SW-13 cells. Growth on C6/36 cells did not reveal a defect in peak virus production (panel iii).
Mutation 3·7 exhibited no defect in 2B/3 cleavage and caused a very small plaque-size (27 % of parent). Fig. 2(d) shows that it was slightly reduced in growth efficiency at 37 °C (panel i) (0·4 log lower peak-titre), and only minimally at 32 °C (panel iii) on SW-13 cells (Fig. 2d
). Mutant 3·22 was not impaired in 2B/3 cleavage but caused a small plaque-phenotype (40 % of parent). Fig. 2(d)
shows that it exhibited a moderate defect in peak virus production at 37 °C (panel ii) (1·5 log reduction) and a profound defect at 32 °C (panel iii) (3 log reduction).
Taken together, these results show that reduced plaque sizes of the mutant viruses which were examined were usually associated with decreased virus production, although the extent of reductions in virus yields were variable among the mutants. For the mutants 3·12 and 3·15, experiments in C6/36 cells did not reveal any evidence of host-restriction of virus production.
Characterization of revertant mutations
During plaque purification of the mutant viruses, plaque-revertant viruses with increased plaque size compared with the original transfection harvests of the mutant viruses, were observed for mutants 2·3, 2·4, 2·5, 2·18, 3·61 and 3·62. To gain insight into whether novel mutations in the NS2B or NS3 proteins might be involved in the revertant phenomena, PCR products derived from the NS2BNS3181 region of these revertant viruses were sequenced. This analysis revealed three classes of mutations associated with plaque reversion (Table 2). Same-site mutations involving different amino acids than the parental residue were observed for two of the revertants of mutant 2·3 (2·3·1 had substitution of residue 47 with glutamic acid instead of the parental arginine and 2·3·3 had substitution of residue 49 with serine instead of the parental aspartic acid); and for the revertant of mutant 2·4 (substitution of residue 54 with valine instead of the parental lysine). Same-site mutations involving the parental amino acid residue occurred for revertants of mutants 3·61 and 3·62, (substitution with parental glutamic acid and aspartic acid residues, respectively). Second-site mutations were observed for one revertant of mutant 2·3, (2·3·2 had substitution of serine for alanine at residue 45, adjacent to the original mutations at residues 47 and 49), and for mutant 2·18, (substitution of a histidine for leucine at residue 122, adjacent to the original mutations at residues 124 and 126). Another type of second-site mutation occurred for the revertant of mutant 2·5, involving substitution of tryptophan for arginine at amino acid residue 62 in the NS3 region.
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Fig. 3(a), panel (i) shows that the parental NS2BNS3181 polyprotein exhibited very efficient cleavage, based on the production of its NS2B and NS3181 cleavage products. This process was mildly inhibited in the presence of microsomal membranes [panel (ii)]. The NS2BNS3181 polyprotein containing the 2·3·2 mutation exhibited a cleavage efficiency in the absence of membranes that closely resembled the parental protease [panel (i)]. In contrast, the 2·3R polyprotein, containing the revertant mutation at position 45 together with the original alanine mutations, was inefficiently cleaved at 20 min, and even by 90 min cleavage yielded less products than the parental protease. In the presence of membranes [panel (ii)], cleavage of the NS2BNS3181 polyprotein containing the 2·3 mutation was slightly less efficient than that of the parental protease, whereas the 2·3R polyprotein was cleaved to only a minor extent. Fig. 3(a)
[panel (ii)] also shows the results for the 2·4 mutation and its revertant. The 2·4 polyprotein was defective in cleavage in the absence of membranes, and the defect was more severe in the presence of membranes. In contrast, the 2·4R polyprotein exhibited more efficient cleavage under both of these conditions.
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Fig. 3(c), panel (i), shows that the NS2BNS3181 polyprotein containing the 2·18 mutation had no apparent cleavage defect in the absence of membranes, whereas the 2·18R polyprotein was markedly impaired. In the presence of membranes, [panel (ii)], the 2·18 polyprotein was only minimally impaired compared to the parent, whereas the 2·18R polyprotein was markedly impaired in cleavage.
Overall, these results indicate that the second-site mutations associated with mutants 2·3, 2·4, 2·5 and 2·18 cause variable effects on the cleavage efficiency of NS2BNS3181 polyproteins. Some (2·4R and 2·5R) improved the cleavage defects caused by the original mutations, whereas others, such as 2·3R and 2·18R, caused deleterious effects.
Effects of reversion mutations on sig2A5356 polyprotein processing
To investigate the effects of reversion mutations on protease-mediated cleavages at other sites in the non-structural polyprotein, pET/BS(+)-sig2A5356 plasmids, encoding both the reversion mutation and the original charged-to-alanine mutation, were constructed and tested for processing of the non-structural polyprotein. Expression of this polyprotein in cells infected with vaccinia virus vTF7-3 allows monitoring of processing events which generate the NS3, NS4A, NS4B and NS5 proteins, and is a surrogate system for analysis of polyprotein processing in virus-infected cells (Chambers et al., 1991). However, the long intervals required for efficient radiolabelling of viral proteins is not amenable to detailed pulse-chase experiments that would allow precise identification of the processing defects caused by mutations. In these experiments, NS4A is not observed (no antiserum is available), and NS5 is not routinely analysed (the antisera react very weakly with the truncated NS5 protein encoded by the plasmid). Only selected mutations that caused small plaques were tested in these experiments. Mutant 2·18 was tested because it had no effect on 2B/3 cleavage and its revertant mutation was very impaired in cleavage of the NS2BNS3181 polyprotein (Fig. 3c
). Mutant 3·15 was tested because it exhibited no significant defect in cleavage of the NS2BNS3181 polyprotein. Cleavage of sig2A5356 polyproteins containing the 2·3 or the 2·5 mutations were also studied, but defects of only a minor nature were observed (data not shown).
Fig. 4(a), shows that the 2·18 mutation caused no change in the production of the NS2B protein compared to the parental polyprotein. There was a slight decrease in the production of NS3 and NS34A related proteins (Fig. 4b
), and the production of the mature form of NS4B was greatly decreased (Fig. 4c
). In contrast, processing of the 2·18R polyprotein containing the 2·18 mutation together with its reversion mutation, yielded levels of NS2B, NS34A and NS4B proteins that were similar to those of the parental polyprotein. These data suggest that the 2·18 mutation causes a defect in processing of the NS3-4A and NS4AB-5 regions, which was compensated by the 2·18R mutation.
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Plaque sizes of engineered revertant viruses
Experiments were also conducted to determine whether the second-site mutations that were associated with plaque reversion could increase the plaque size of the small plaque-mutant viruses from which they were originally derived. YF viruses were engineered to contain a portion of the NS2BNS3181 region encompassing the original charged-to-alanine mutation and the associated reversion mutation. This allowed direct testing of the effects of these mutations in the YF5·2iv genetic background, in the absence of mutations outside of the NS2BNS3181 region that might have accumulated during isolation of the original mutants. If an increase of plaque size could be demonstrated in such cases, this would suggest that the reversion mutations within the NS2BNS3181 region contributed compensatory effects during replication of the original mutant virus. For the original 2·5 mutant, the plaque size was 39 % of parental size (Table 1). The plaque size of the virus containing the 2·5 mutation together with the substitution of tryptophan for histidine at NS3 position 62 was 85 % of parental size. For the original 2·18 mutant, the plaque size was 22 % of parental size (Table 1
). Virus containing the 2·18 mutation together with the substitution of histidine for leucine at NS2B position 122 gave a plaque size of 70 % of the parental size. These results are consistent with a compensatory effect of the 2·5R and 2·18R mutations on the defect in virus plaque-formation associated with the 2·5 and 2·18 mutations, respectively.
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DISCUSSION |
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In the case of the 2·3 mutation, which targeted a charge cluster at the proximal end of the conserved domain of NS2B, a defect in cleavage of the NS2BNS3181 polyprotein in the presence of membranes was observed, and subtle defects in processing of other non-structural cleavage sites were observed. Several reversion mutations were mapped to the same site or a site adjacent to the original mutation, involving charged (glutamic acid) or uncharged polar (serine) amino acid substitutions. These findings suggest that the interaction of a NS2B with NS3 depends on a charge cluster at positions 47 and 49 of NS2B, presumably through effects on complex formation, and consistent with previous studies (Chambers et al., 1993). In the absence of the charge interactions, the serine substitutions at positions 45 and 49 might promote binding of NS2B to NS3 as a result of hydrogen bond interactions of their hydroxyl groups with residues in the binding cleft on NS3 (see below). Cell-free cleavage of the NS2BNS3181 polyprotein revealed that the 2·3R mutation was defective in cleavage compared with 2·3, and thus 2B/3 cleavage efficiency did not correlate with plaque size for the 2·3 mutant and its revertants. However, this assay may not accurately reflect processing of this site in the context of a full-length non-structural polyprotein, where interactions of multiple viral and host proteins could result in different effects at the 2B/3 and other cleavage sites when comparing mutant and revertant proteases.
The 2·18 mutation was associated with defects in the production of NS34A polyproteins and NS4B from the sig2A5356 polyprotein. This observation suggests that the interaction of the protease complex with the polyprotein substrate during the cleavages at the 3/4A, and 4B/5 cleavage sites may be impaired. A second-site mutation associated with the 2·18 mutation partially restored the polyprotein processing defects, as well as led to an increase in the plaque forming capacity of the corresponding mutant virus. The proximity of the reversions to the original mutation suggests that its effects may be mediated through preservation of a charge cluster involved in local structural integrity or membrane association of NS2B. However, the observation that cleavages affecting the production of NS34A and NS4B were primarily affected suggests that the mutations and reversions may also cause effects on substrate binding in the downstream region of the polyprotein.
Introduction of the 2·18R mutation together with the original 2·18 mutation into the YF5·2iv infectious clone yielded virus with a plaque size larger than that of the 2·18 mutant itself. This suggests that the improvement in polyprotein processing associated with the revertant substitution contributes to more efficient virus replication. Although cleavage efficiency of the 2·18R mutation at the 2B/3 cleavage site (Fig. 3c) did not correlate with the ability of this mutation to affect plaque size, the cell-free cleavage assay of the NS2BNS3181 polyprotein may not accurately reflect the processing of this site in the context of a full-length non-structural polyprotein, as discussed for the 2·3 and 2·3R mutations. In support of this, results shown in Fig. 4
indicate that the 2·18R mutation does not in fact compromise production of NS2B, as suggested by the cell-free cleavage assay (Fig. 3c
).
For the 3·15 mutation, the cleavage defects included a decreased cleavage of the NS2AB protein and reduced production of NS3 and NS34A-related proteins. These results are consistent with a deleterious effect of this mutation on the interaction of the NS2BNS3181 complex with the 2A/2B, 3/4A, and 4A/4B cleavage sites, more than the 2B/3 or 4B/5 sites. This may result from a specific interaction of the three charged residues targeted by the mutation with the substrate contacts in the 3/4A and 2A/2B regions, which differ from interactions at the 2B/3 and 4B/5 cleavage sites. Since no second-site mutation was available for the 3·15 mutation, no further explanation of its cleavage defect can be given at this time.
The 2·5 mutation was characterized by a reduced level of 2B/3 cleavage efficiency. This mutant had a second-site mutation in a region of the NS3 protease that, based on the 3D structure of dengue-2 protease, has been implicated as part of the binding site for its NS2B cofactor (Matusan et al., 2001). In that study, residues KRIE6366 in the dengue-2 NS3 protease were predicted to be solvent-exposed and likely to make contact with the N-terminal portion of the conserved domain of NS2B, which corresponds to the location of mutation 2·5. To gain insight into the relationship between the 2·5 mutation and its NS3 reversion mutation, we derived a homology model for the YFV NS3 protease and analysed the effects of a tryptophan substitution at position 62 (Fig. 5
). Using predictions for the dengue-2 virus structure as a guide (Matusan et al., 2001
), tryptophan is predicted to interact with the alanine substitution at position 55 in NS2B. In support of this, comparison of sequence alignments of 12 flavivirus sequences showed that only Langat, tick-borne encephalitis and Powassan viruses have non-polar residues at residue 62 in NS3 (YF numbering), and a hydrophobic residue (tryptophan) at position 55 of the YFV NS2B (data not shown). In contrast, all other flaviviruses have hydrophilic residues, (either arginine or lysine) at position 55. Only in YFV is an arginine in NS3 paired with a lysine in NS2B. Although both of these residues carry positive charges, a van der Waals-type interaction may occur between them. Replacement of lysine by alanine at NS2B position 55 would create some empty space (four methylene groups) and substitution of the more bulky tryptophan for arginine at NS3 position 62 would fill the space and retain hydrogen bonding ability, through the side chain of tryptophan. Our hypothesis is that lysine, leucine and glutamic acid at positions 55, 56 and 58 of NS2B bind in a pocket on NS3 lined by surrounding hydrophobic and non-polar residues (leucine at positions 20 and 67, isoleucine at position 24, glycine at positions 82 and 83). An interaction of tryptophan at NS3 position 62 with alanine at NS2B position 55 may be stabilized due to effects of this hydrophobic contact region. According to this model, the 2·5R mutation improves binding interactions in the hydrophobic pocket, leading to improved protease cleavage activity and contributing to more efficient virus replication.
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The observation that no second-site revertants could be obtained from mutations in the NS3 region, together with the fact that most lethal alanine substitutions occurred in NS3, may indicate a strong selection against mutations which perturb the conserved structure of this domain, and a low tolerance for secondary mutations, which might otherwise provide compensatory effects. In contrast to NS3, mutations may be more readily tolerated in NS2B, which may undergo a dynamic interaction with the loosely structured amino terminus of NS3, as appears to be the case for the NS3 protease of hepatitis C virus (Satoh et al., 1995; Love et al., 1998
).
In conclusion, our results suggest the existence of proteinprotein interactions among the NS2BNS3 protease and non-structural proteins that affect folding of the polyprotein and access of the protease to the non-structural cleavage sites. Further experiments, such as trans cleavage assays of mutant and revertant NS2BNS3 proteases and substrate polyproteins, as well as mutagenesis of regions surrounding the cleavage sites, which are inefficiently cleaved in the presence of the protease mutations, may be of interest. These should reveal more details of the molecular determinants governing normal processing of the YFV non-structural polyprotein.
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ACKNOWLEDGEMENTS |
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Received 7 July 2004;
accepted 13 January 2005.