Genetic Interaction of Flavivirus Nonstructural Proteins NS1 and NS4A as a Determinant of Replicase Function

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Journal of Virology, June 1999, p. 4611-4621, Vol. 73, No. 6
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Genetic Interaction of Flavivirus Nonstructural Proteins NS1 and NS4A as a Determinant of Replicase Function

Brett D. Lindenbach and Charles M. Rice^*

Department of Molecular Microbiology, Washington University School of Medicine, St. Louis, Missouri 63110-1093

Received 11 January 1999/Accepted 24 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Nonstructural protein 1 (NS1) of yellow fever virus (YF) is a glycoprotein localized to extracytoplasmic compartments withininfected cells. We have previously shown that NS1 can be suppliedin trans and is required for viral RNA replication, a processthought to occur in membrane-bound cytoplasmic complexes. Herewe report that the NS1 gene from a related virus, dengue virus(DEN), is unable to function in the process of YF RNA replication.This virus-specific incompatibility leads to a lack of initialminus-strand accumulation, suggesting that DEN NS1 is unable toproductively interact with the YF replicase. Based on a YF deletionmutant that requires NS1 in trans, a genetic screen for suppressormutants was used to select virus variants able to utilize DENNS1. In three independent selections, a single mutation was mappedto the NS4A gene, which encodes a putative transmembrane replicasecomponent. This mutation, as well as several additional mutations,was engineered into the NS1-deficient genome and confirmed a geneticinteraction between NS1 and NS4A. These findings suggest a potentialmechanism for integrating NS1 into the cytoplasmic process ofRNAreplication.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Replicases of eukaryotic positive-strand RNA viruses have intricate relationships with cellular membranes, a fact which oftencomplicates their detailed analysis. Nevertheless, impressiveadvances have been made in understanding the structure and functionof several viral replicases (18, 19, 53). We have been investigatingthe replication of yellow fever virus (YF), which also utilizesa membrane-bound replicase (10, 17). YF is the prototype forthe flaviviruses, an important group of human pathogens that includesdengue virus (DEN), Japanese encephalitis virus, and tick-borneencephalitis virus. In this paper, we reveal a genetic interactionthat exists between a flavivirus protein residing in the secretorypathway and a membrane protein postulated to be part of the viralreplicase and show that this interaction is crucial for the processof flavivirus RNAreplication.

The flavivirus genome consists of an ~11-kb, single-stranded RNA molecule of positive polarity (36). This RNA is cappedat its 5' end and serves as the mRNA for the translation of alarge polyprotein. Mature viral proteins are processed from thisprecursor by a viral serine protease and multiple host proteinases(34). The virion structural components are encoded in the 5'one fourth of the genome, while viral nonstructural (NS) proteinsare encoded in the remainder of the genome. The overall gene orderis C-prM-E-NS1-NS2A-NS2B-NS3-NS4A-NS4B-NS5. The major functionof NS proteins is the replication of viral RNA, and several relevantactivities have been mapped to NS proteins. NS5 is the RNA-dependentRNA polymerase as well as a putative methyltransferase thoughtto be involved in the formation of the RNA cap (6, 46). TheN-terminal region of NS3 contains the catalytic residues of theviral serine protease, which requires the protein cofactor NS2Bfor activity (9, 15). The remainder of NS3 comprises an RNAtriphosphatase, which may contribute to RNA capping (49), aswell as an RNA helicase with nucleoside triphosphatase activity(16, 48). Several other NS proteins (NS2A, NS4A, and NS4B)are small hydrophobic proteins with unknown functions, althoughit has been suggested that they may serve to anchor the viralreplicase to cellular membranes (8).

NS protein 1 (NS1) is inserted into the endoplasmic reticulum (ER) by a signal sequence located in the C terminus of the Eprotein and is processed by host signal peptidase (13). Shortlyafter synthesis, NS1 is cleaved from NS2A by an unknown ER-residenthost proteinase (14). NS1 is a glycoprotein that forms homodimersand interacts with membranes via an unknown mechanism (42, 51,52). It is largely retained within the cell, where it has beenlocalized to presumed sites of RNA replication (26, 50). Asignificant proportion of NS1 is also secreted, and a minor amountassociates with the cellsurface.

The flavivirus genome is replicated via a minus-strand intermediate that continues to accumulate over the course of infection,although the ratio of plus-strand RNA to minus-strand RNA maychange over time (12). Despite its extracytoplasmic localization,NS1 is an essential component of the viral replicase. Definedmutations in NS1 can result in dramatic decreases in the levelof viral RNA accumulation, and such mutations provided the firstfunctional data indicating that NS1 is involved in this process(29, 30). We have recently demonstrated that a YF genome bearinga large in-frame deletion in the NS1 gene, YF $Delta$ SK, is severelydefective in viral replication (25). In order to study thisdefect, we demonstrated that YF $Delta$ SK could be complemented in transby the expression of a functional NS1 gene via a noncytopathicSindbis virus vector. This strategy permitted the analysis ofYF $Delta$ SK replication with or without trans complementation. YF $Delta$ SKrequired NS1 for growth, plaque formation, and RNA replication.Examination of early events in RNA replication revealed a requirementfor NS1 prior to or at initial minus-strandsynthesis.

The objective of this investigation was to analyze the ability of a heterologous NS1 gene to function in the trans complementationof YF $Delta$ SK. We initially found that YF $Delta$ SK did not complete earlyminus-strand synthesis in cells expressing DEN NS1 and thus wasnot complemented by DEN NS1 supplied in trans. These results ledus to hypothesize that NS1 requires interactions with other replicasecomponents for function and that these interactions might be virusspecific. Based on this hypothesis, we undertook a genetic screenfor YF $Delta$ SK suppressor mutants able to overcome this block in replication.The results presented here indicate that a single position inNS4A can influence the ability of YF $Delta$ SK to utilize DENNS1.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell cultures, virus stocks, and plaque assays. BHK-21 cells were transfected with pSINrep21 DNAs by use of Lipofectamine (Life Technologies, Inc., Gaithersburg, Md.) andselected with media containing puromycin (Sigma, St. Louis, Mo.)essentially as described previously (1). BHK-SINrep21 cellswere cultured in minimal essential medium (Life Technologies)containing 7.5% fetal calf serum, nonessential amino acids, and5 µg of puromycin per ml at 37°C in 5% CO₂.

YFs were propagated by low-multiplicity passage (multiplicity of infection [MOI], <0.1) for 36 to 48 h. Virus culture mediawere clarified by centrifugation (3,000 × g for 10 min), dividedinto aliquots, and stored at $-$ 80°C. DEN type 2 (DEN-2) strainPR-159(S1) (kindly provided by Ellen Strauss, California Instituteof Technology) was amplified by low-multiplicity passage on C6/36cells in minimal essential medium containing 10% heat-inactivatedfetal calf serum for 5 days at 30°C in 5% CO₂. Plaque assays weredone as previously described (25), except that DEN plaques wereallowed to develop on BHK-21 cells for 4days.

For plaque purification of viruses, cells were overlaid with minimal essential medium containing 2% fetal calf serum and 1%SeaPlaque agarose (FMC BioProducts, Rockland, Maine) and allowedto incubate for 3 days. Plaques were visualized by 3 h of incubationwith phosphate-buffered saline (PBS) containing 0.012% neutralred (Sigma). Plaques were picked with a sterile 1-ml pipette tipand resuspended in fresh media, and viruses were eluted from theagarose at 4°C for 4 h. The eluate was diluted and used for anotherround of plaque formation and picking. The final eluate was amplifiedin the appropriate cell type and stored. We found that for efficientamplification of the final eluate, it was necessary to removethe inoculum following adsorption by washing the cells a few timeswith PBS, perhaps due to the toxicity of neutralred.

Plasmid constructions. Standard molecular biology techniques were used (2, 40). The structures of all plasmids were checked by sequencing andrestriction analysis. pSINrep21 is a DNA plasmid containing thegenome of a noncytopathic SINrep vector under the transcriptionalcontrol of the Rous sarcoma virus 5' long terminal repeat promoter(1, 25). pSINrep21/DEN NS1 was constructed as follows. TheDEN NS1 signal sequence and the NS1-2A genes [DEN PR-159(S1) codons754 to 1345] were amplified from pDEN 32 (a kind gift from YoungHahn, University of Virginia Health Science Center) by PCR (forwardprimer, 5'-GCGTCTAGAACATGTCACTGTCTGTGTCACTGG-3'; reverse primer,5'-GCGAGCTCCTAGGTTAGCTCCTTTTCTTGCTGG-3') and cloned into the XbaIand SacI sites of pBSIISK $-$ to yield pBSII/DEN NS1-2A. The DENNS1 gene was subcloned as a 1,131-bp XbaI-blunted MspI fragment,prepared by use of mung bean nuclease, into the XbaI/PmlI sitesof pSINrep21. This procedure introduced an in-frame terminationcodon precisely after the DEN NS1 gene as well as a novel DraIIIsite.

pSINrep21/DEN NS1-2A was constructed via a three-piece ligation with a 6,652-bp BsrGI/Bsp120I fragment of pSINrep21/DEN NS1,a 5,441-bp PmlI/BsrGI fragment of pSINrep21, and an 839-bp Bsp120I/Ecl136IIfragment of pBSII/DEN NS1-2A.

We have recently participated in the construction of a stable full-length infectious YF clone by subcloning the YF genomicregions into a low-copy-number plasmid (4). This construct,pACNR/FLYF, gave rise to RNA that had a greater specific infectivitythan that from the previously described two-plasmid system (35),most likely due to the greater efficiency of preparing high-qualitytemplates for transcription. Virus stocks derived from this constructwere indistinguishable from several YF 17D strains by multiplecriteria. Therefore, pACNR/YF $Delta$ SK was constructed by use of thecommon NsiI and AatII sites of pYFM $Delta$ SK (25) and pACNR/FLYF.Derivatives of this plasmid containing mutations in NS4A wereconstructed as follows. To reconstruct the NS4A-N42Y (A5783T)mutation, pYFM $Delta$ SK was amplified with Pfu DNA polymerase and mutagenicprimers (5'-GCTTACCGCTATGCACTATCA-3' and 5'-CGAATGGCGATACGTGATAGT-3'[mutated sites are underlined in these and subsequent primers]),followed by DpnI digestion of the wild-type plasmid. The mutatedregion was then subcloned into pACNR/YF $Delta$ SK by use of the commonStuI and NgoMIV sites. To facilitate further mutagenesis of NS4A,an intermediate construct was made by subcloning the NheI/SphIregion of pACNR/FLYF into the XbaI/SphI sites of pNEB193 (NewEngland Biolabs, Beverley, Mass.). This construct was mutatedas described above with primers having the sequences 5'-AAGGCTCTAGAGCTTACCGCCATGCACTATCGATGATGCCTGA-3'and 5'-CAGGCATCATCGATAGTGCATGGCGGTAAGCTCTAGAGCCTT-3'. The resultingconstruct, pNEB/YF5459-6897H, contained the NS4A-N42H mutationflanked by silent mutations introducing novel XbaI and BspDI sites.The StuI/NgoMIV fragment of this construct was subcloned intopACNR/YF $Delta$ SK as described above. Additional NS4A mutations wereconstructed by cloning annealed oligonucleotides into the XbaI/BspDIsites of pNEB/YF5459-6897H, followed by subcloning the StuI/NgoMIVfragment as describedabove.

The oligonucleotides used for mutagenesis were as follows: NS4A-N42F, 5'-CTAGAGCTTACCGCTTTGCACTAT-3' and 5'-CGATAGTGCAAAGCGGTAAGCT-3';NS4A-N42W, 5'-CTAGAGCTTACCGCTGGGCACTAT-3' and 5'-CGATAGTGCCCAGCGGTAAGCT-3';NS4A-N42Y2, 5'-CTAGGGCTTATAGGTACGCTCTGT-3' and 5'-CGACAGAGCGTACCTATAAGCC-3';NS4A-N42Q, 5'-CTAGAGCTTACCGGCAGGCACTAT-3' and 5'-CGATAGTGCCTGCGCGGTAAGCT-3';NS4A-N42D, 5'-CTAGAGCTTACCGCGACGCCCTAT-3' and 5'-CGATAGGGCGTCGCGGTAAGCT-3';NS4A-N42M, 5'-CTAGAGCCTACAGGATGGCATTAT-3' and 5'-CGATAATGCCATCCTGTAGGCT-3';and NS4A-N42S, 5'-CTAGAGCTTACAGATCTGCACTAT-3' and 5'-CGATAGTGCAGATCTGTAAGCT-3'.

RNA transcriptions and transfections. RNA transcripts were synthesized in reaction mixtures containing 40 mM Tris (pH 7.9); 6 mM MgCl₂; 2 mM spermidine-HCl₃; 1mM each UTP, GTP, CTP, and ATP; 0.6 mM cap analog [^m7G(5')ppp(5')G; New England Biolabs]; ~0.5 µM [5,6-³H]UTP (1.0 mCi/ml, 50 Ci/mmol; New England Nuclear Corp., Boston,Mass.); 10 mM dithiothreitol; 16 U of RNasin (Promega, Madison,Wis.); 20 U of SP6 RNA polymerase (Epicentre, Madison, Wis.);and 100 ng of XhoI-linearized template DNA. Nucleotide utilizationwas monitored by measuring [5,6-³H]UTP incorporation via RNA adsorption to DE-81 (Whatman, Maidstone,United Kingdom) filter paper (40). Cells were electroporatedwith RNAs essentially as described previously (25) on a modelT820 square wave generator (BTX Inc., San Diego, Calif.). To measureRNA infectivity by infectious-center assays, cells were electroporatedwith 1 µg of RNA, serially diluted, and mixed with 5 × 10⁵ untransfected cells to serve as substrates for plaque formation.Cells were allowed to adhere to 35-mm dishes for 4 to 6 h beforecell monolayers were overlaid with agarose-containing medium asdescribedabove.

RNA analysis. Analysis of viral RNA accumulation was performed with an RNase protection assay (RPA) as previously described (25). Foranalysis of early minus-strand accumulation, cells were synchronouslyinfected at 4°C, the inocula were removed by extensive washingin the cold with chilled PBS, and infections were initiated bythe addition of warm media. At various times postinfection, totalcellular RNAs were extracted with Trizol (Life Technologies) andanalyzed with a two-cycle RPA (31). Synthetic minus-strand standardswere added directly to separate mock-infected cell lysates duringthe extraction procedure in order to determine the sensitivityof the extraction and detection methods as well as to serve asquantitationmarkers.

Protein analysis. Cells were labeled in methionine- and cysteine-deficient Dulbecco's modified Eagle medium (Life Technologies) containing 2%fetal calf serum and Expre³⁵S³⁵S protein labeling mix (100 µCi/ml; New England Nuclear Corp.)for 3 h. Cells were lysed in 50 mM Tris (pH 7.5)-1 mM EDTA-0.5%sodium dodecyl sulfate (SDS), and DEN NS1 was immunoprecipitatedessentially as described previously (7) with monoclonal antibody3E9 (a kind gift from Robert Putnak, Walter Reed Army Instituteof Research) and Pansorbin (Calbiochem, San Diego, Calif.). Theamount of antibody used in immunoprecipitations was shown to besaturating in pilot experiments testing different antibody dilutions.Proteins were resolved on an SDS-10% polyacrylamide gel priorto fluorographic treatment and exposure tofilm.

Viral sequence and computational analyses. Viruses were pelleted with polyethylene glycol 8000 as previously described (25), and RNAs were extracted with Trizol. cDNAswere synthesized with Superscript II reverse transcriptase (LifeTechnologies) and amplified by PCR with internal primer pairs.Following silica gel purification (Qiagen Inc., Chatsworth, Calif.),PCR products were used directly in BigDye cycle sequencing reactions(Perkin-Elmer, Foster City, Calif.) run on a model ABI 377 electrophoresisunit (Perkin-Elmer). Sequences were interpreted and assembledwith Lasergene software (DNAStar, Madison, Wis.) by use of atleast two overlapping reactions in each direction. Sequence changeswere confirmed by ThermoSequenase cycle sequencing reactions (AmershamInc., Arlington Heights, Ill.) and manualelectrophoresis.

Computer predictions of NS4A topology and secondary structure were based on an alignment of 63 flavivirus NS4A coding regionsobtained from the PFAM database (43). Structural predictionswere made via the EMBL-Heidelberg PHD server (37-39). The threadingof NS4A (see Fig. 8A) was based on the refined output of PHDRhtm,which has an expected average accuracy of >82% at each position.Secondary-structure predictions were the refined output of PHDsecbased on an expected average accuracy of >82%. However, as thisneural network was trained on water-soluble globular proteins,the accuracy of the NS4A secondary-structure prediction isindeterminable.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression of DEN NS1. Populations of BHK-21 cells expressing the NS1 or NS1-2A gene from DEN-2 strain PR-159(S1) were derived by use of the pSINrep21vector, which has previously been used to express the homologousregions of YF. In order to discriminate between the two flavivirusNS1 genes, we refer to them as DEN NS1 and YFNS1.

The patterns of DEN NS1 expression by metabolically labeled BHK-SINrep21 cells or DEN-2-infected cells were examined by immunoprecipitation,separation by SDS-polyacrylamide gel electrophoresis, and fluorography(Fig. 1). The major cell-associated form of DEN NS1 migrated asa single band of 48 kDa after boiling (Fig. 1, lanes 1, 3, and4) or as a dimeric form of about 84 kDa in unboiled samples (lanes9 to 11). Conditioned media from these cells contained secretedforms of DEN NS1 which migrated as a ladder of bands in the rangeof 50 to 53 kDa (boiled, Fig. 1, lanes 5, 7, and 8) or 90 to 96kDa (not boiled, lanes 12 to 14) and representing products ofadditional glycan processing. Small amounts of the slower-migratingforms were also found to be cell associated and were most likelyDEN NS1 destined for secretion. In addition, a minor band of 63kDa, which may be uncleaved NS1-2A, was associated with DEN-2-infectedcells. The secretion of DEN NS1 from BHK-SINrep21 cells appearedto be more efficient than that from DEN-2-infected cells. Thisfinding may represent a specific retention of DEN NS1 by the DEN-2replication machinery or may result from the disruption of secretorypathway function during viral infection. These data suggest thatpSINrep21-expressed DEN NS1 and DEN NS1-2A were processed, glycosylated,and targeted for secretion in a manner similar to that of authenticDEN NS1.

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FIG. 1. Expression of DEN NS1 and NS1-2A. BHK-21 cells (mock infected or infected with DEN-2 [MOI, 10] for 22 h) or BHK-SINrep21 derivatives were metabolically labeled for 3 h. NS1 was immunoprecipitated from equivalent portions of cellular SDS extracts or conditioned labeling media and eluted into loading buffer. Half of the eluate was boiled prior to electrophoresis. Numbers to the left indicate relative molecular masses in kilodaltons.

Protein band intensities should reflect the relative abundance of labeled proteins, since immunoprecipitations were performedwith an excess of antibodies. The amount of pSINrep21-expressedDEN NS1 was about twofold smaller than the amount expressed incells infected with DEN-2 from 22 to 25 h postinfection, whenviral replication is expected to be exponential. Parallel analysisof [³⁵S]Cys- and [³⁵S]Met-labeled BHK-SINrep21 cells expressing DEN NS1 or YF NS1revealed similar NS1 band intensities (data not shown). Giventhat both flavivirus NS1 genes contain 12 Cys and 9 Met residues,the amounts of DEN NS1 and YF NS1 expressed by pSINrep21 werecomparable. These data suggest that the quantities of DEN NS1expressed by BHK-SINrep21 cells were likely to be sufficient forit to function in transcomplementation.

DEN NS1 does not support YF $Delta$ SK. YF $Delta$ SK is a YF genome containing a large in-frame deletion in the NS1 gene. We have previously demonstrated that this virusis severely defective in RNA replication and growth but can becomplemented in trans by the expression of YF NS1 or YF NS1-2A(25). In the current report, we used two methods of generatingYF $Delta$ SK. As previously described, YF $Delta$ SK was originally constructedby use of a YF infectious clone residing in two separate plasmidsthat can be ligated together to produce a full-length templatefor RNA transcription (35). This method yielded YF $Delta$ SK RNAs witha moderate specific infectivity (~10³ PFU/µg of RNA). In addition, YF $Delta$ SK was reconstructed in the contextof a recently developed stable full-length YF infectious cloneto produce pACNR/YF $Delta$ SK (see Materials and Methods). Transcriptionof the resultant plasmid yielded highly infectious YF $Delta$ SK RNAsthat were dependent on the expression of YF NS1 in trans for RNAreplication and virus growth (see below; data notshown).

To assess the ability of DEN NS1 to trans complement YF $Delta$ SK, we examined YF $Delta$ SK plaque formation on cells expressing DEN NS1,YF NS1, or green fluorescent protein (GFP). Our original stocksof YF $Delta$ SK were derived from the two-plasmid clone of the deletionmutant and had plaque titers of 3 × 10⁶ to 4 × 10⁶ PFU/ml on YF NS1-expressing cells and <5 PFU/ml on DEN NS1- orGFP-expressing cells, indicating that DEN NS1 was not capableof supporting YF $Delta$ SK plaqueformation.

The growth of YF $Delta$ SK in YF NS1- and DEN NS1-expressing cells in several independent single-cycle growth experiments was monitored.In all cases, the growth of YF $Delta$ SK was not detected in cells expressingDEN NS1, while cells expressing YF NS1 were able to support thegrowth of this virus. A representative experiment is shown inFig. 2A. At 0 h postinfection, similar levels of input virus werepresent in both cultures. The titers of YF $Delta$ SK increased over timein BHK-SINrep21/YF NS1 cells, demonstrating viral growth via transcomplementation. By 23 h postinfection, the cytopathic effectsof viral replication had eliminated a majority of these cells,and the decrease in viral titers after 23 h probably representsinactivation of the virus under the conditions of incubation.In contrast, no detectable increase in viral titers was seen forDEN NS1; only the decay of the initial inoculum was seen. Notethat the decay of virus occurred with similar kinetics in bothcultures. In this particular experiment, a large amount of residualinfectivity was present at early times, most likely due to insufficientwashing of the cells, which could have obscured low levels ofYF $Delta$ SK growth. However, in other experiments, the input inoculumwas removed by more extensive washing to below the limit of detectionused in the plaque assays (typically 50 PFU/ml). In these experiments,the level of YF $Delta$ SK remained below detectable levels in BHK-SINrep21/DENNS1 cells, confirming an inability to grow in these cells (datanot shown). Similar experiments also demonstrated the inabilityof DEN NS1-2A to support the growth of YF $Delta$ SK. Because YF NS1-2Awas less efficient at complementing YF $Delta$ SK (25), further studieswith DEN NS1-2A were not pursued. These data indicated that NS1was functioning in a flavivirus-specific manner.

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FIG. 2. DEN NS1 does not complement YF $Delta$ SK. (A) Growth of YF $Delta$ SK on cells expressing DEN NS1 (

) or YF NS1 ( $black-lozenge$ ). Cells were infected with YF $Delta$ SK (MOI, 10) for 1 h. The inoculum was removed, the cells were briefly rinsed with PBS, and fresh growth medium was added. Virus growth media were sampled at 0, 12.5, 23, 37, and 46 h postinfection, clarified, and stored at $-$ 80°C. Virus titers were determined on BHK-SINrep21/YF NS1 cells and plotted here on a semilogarithmic scale. (B) RPA of viral minus strands. RNAs were harvested at 0, 4, 8, or 20 h postinfection. Equivalent portions of protected minus-strand reactions were subjected to denaturing electrophoresis, dried, and exposed to film. Numbers above lanes 2 to 5 refer to the numbers of synthetic minus-strand molecules analyzed in parallel; numbers above lanes 6 to 19 refer to hours postinfection. The 10⁹ standard, which appeared as a smear in this exposure, did yield a distinct band in a lighter exposure and is included here to further demonstrate the sensitivity of this assay to the quantity of input RNA.

YF NS1 was previously shown to be required for very early events of RNA replication. To determine if trans complementationwith DEN NS1 was blocked in these early events, the accumulationof YF $Delta$ SK minus-strand RNA was monitored with a sensitive strand-specificRPA. BHK-SINrep21 cells (2 × 10⁶/well) expressing DEN NS1, YF NS1, or GFP were synchronously infectedat an MOI of 10, and total cellular RNAs were extracted at specifictimes postinfection for analysis. In addition, in vitro-synthesizedminus strands were added to uninfected cell lysates during RNAextraction to serve as quantitation standards, and the levelsof a cellular mRNA encoding glyceraldehyde-3-phosphate dehydrogenase(GAPDH), were examined as a loading control. As shown in Fig.2B, a background level of YF minus strands was detected immediatelyfollowing infection; this level most likely represents a smallamount of YF minus strands present in the virus preparation, consistentwith our previous results (25). Following infection, YF minusstrands accumulated over time in BHK-SINrep21/YF NS1 cells (Fig.2B, lanes 11 to 14). Based on the quantitation standards (Fig.2B, lanes 2 to 6) and the amount of infectious input virus, thefirst YF $Delta$ SK minus strands appeared to accumulate between 4 and8 h postinfection in cells expressing YF NS1, consistent withearlier findings (25). Furthermore, minus-strand accumulationrequired the expression of NS1, as no increase in signal was seenin cells expressing GFP (Fig. 2B, lanes 15 to 19). Cells expressingDEN NS1 also failed to show any accumulation of YF $Delta$ SK minus strands,even by 20 h postinfection. Taken together, these data indicatethat DEN NS1 is unable to support the growth of YFd $Delta$ SK due toa block prior to or at initial minus-strandsynthesis.

Selection of YF $Delta$ SKden variants. We wondered whether we could use these observations to drive the selection of YF $Delta$ SK variants able to utilize DEN NS1. YF $Delta$ SKRNAs transcribed from pACNR/YF $Delta$ SK were transfected into BHK-SINrep21/DENNS1 cells. We reasoned that the majority of YF $Delta$ SK RNAs would notbe complemented by DEN NS1, while those rare RNAs containing changesallowing them to utilize DEN NS1 would be complemented in transand should therefore replicate. In one representative experiment,BHK-SINrep21 cells expressing YF NS1, DEN NS1, or GFP (~2 × 10⁶ each) were electroporated with 4 µg of YF $Delta$ SK RNA, and a portionof the cells was plated on 100-mm dishes. At 50 h posttransfection,the media were recovered for analysis and the cell monolayerswere stained with crystal violet. As shown in Fig. 3, nearly allcells expressing YF NS1 were destroyed by the cytopathic effectsof YF $Delta$ SK replication, while cells expressing GFP were unaffecteddue to the lack of a functional NS1 gene. Surprisingly, comet-formplaques appeared on cells expressing DEN NS1, suggesting the replicationand spread of YF $Delta$ SK within these cells. The variable shapes andsizes of these plaques were likely due to the use of a liquidoverlay on the plates. When dilutions of cells from these sametransfections were overlaid with a semisolid medium, DEN NS1-expressingcells yielded a small number of plaques that were heterogeneousin size. The specific infectivity of YF $Delta$ SK RNA was 3 × 10³ PFU/µg in this cell type. Transfection of this same RNA intoYF NS1-expressing cells yielded large round plaques at a specificinfectivity of 9 × 10⁵ PFU/µg. Thus, only a small fraction of the YF $Delta$ SK RNA was capableof replicating in DEN NS1-expressing cells.

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FIG. 3. Selection of YF $Delta$ SKden by RNA transfection. BHK-SINrep21 cells expressing YF NS1, DEN NS1, or GFP were transfected with YF $Delta$ SK RNA and plated on 100-mm dishes. Following incubation, the cells were fixed and stained for plaque formation.

The conditioned media from these transfected cells were tested for plaque formation on cells expressing DEN NS1 or YF NS1(Table 1). YF $Delta$ SK that was initiated in cells expressing YF NS1had a high plaque titer on cells expressing YF NS1 but did notproduce plaques on cells expressing DEN NS1. This result confirmedthat YF $Delta$ SK was not complemented by DEN NS1. However, transfectionof cells expressing DEN NS1 yielded YF $Delta$ SK capable of forming plaqueson both YF NS1- and DEN NS1-expressing cells. The amount of virusproduced by the DEN NS1-expressing cells was less than that producedby the YF NS1-expressing cells, a result which most likely reflectedthe difference in specific infectivities. Note that the titersof the DEN NS1-initiated virus were similar on both types of cells,suggesting that a given virus particle might be capable of infectingeither cell type. Passage of the DEN NS1-initiated virus on YFNS1-expressing cells yielded similar virus titers on both celltypes (data not shown), further supporting this hypothesis andalso demonstrating that the ability to form plaques on DEN NS1-expressingcells was retained after passage. Thus, not only was there a differencein YF $Delta$ SK RNA specific infectivity between these two cell types,but also the resultant viruses exhibited a large quantitativedifference in their ability to form plaques on these cell types.These results indicated that there were two YF $Delta$ SK populations:YF $Delta$ SK, which can replicate only in YF NS1-expressing cells, anda minor population able to replicate in either YF NS1- or DENNS1-expressing cells. We termed this latter virus YF $Delta$ SKden.

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TABLE 1. YF $Delta$ SK produced by transfected cells

From a genetic standpoint, it appeared that viruses with the YF $Delta$ SKden phenotype were variants of YF $Delta$ SK that had gained theability to utilize DEN NS1 for replication. If indeed YF $Delta$ SKdenwas a subpopulation of YF $Delta$ SK, it should also have been possibleto select YF $Delta$ SKden from the larger population by passage on DENNS1-expressing cells. This idea was examined in several experimentswith a YF $Delta$ SK stock that had been initiated from pACNR/YF $Delta$ SK inYF NS1-expressing cells. This virus stock had a titer of 2 × 10⁷ PFU/ml on YF NS1-expressing cells and undetectable infectivities(<5 PFU/ml) on DEN NS1- and GFP-expressing cells. These threecell types were infected for 1 h with the same amounts of virusto yield an MOI of 10 on YF NS1-expressing cells, the cells werewashed, and virus accumulation was monitored over time. The accumulationof YF $Delta$ SK was detected by plaque formation on YF NS1-expressingcells (Fig. 4A). YF $Delta$ SK produced robust growth on YF NS1-expressingcells and undetectable growth on GFP-expressing cells. After ashort lag, modest growth was seen on DEN NS1-expressing cells.The accumulation of YF $Delta$ SKden in these same samples was monitoredby plaque formation on DEN NS1-expressing cells (Fig. 4B). Incontrast to the high titer of YF $Delta$ SK produced by YF NS1-expressingcells, the titer of YF $Delta$ SKden remained below the detection limitof this assay on DEN NS1-expressing cells. Note that in the sampletaken at 36 h postinfection, there was a difference in infectivityof at least 7 orders of magnitude between BHK-SINrep21/YF NS1and BHK-SINrep21/DEN NS1 cells (Fig. 4). As predicted, YF $Delta$ SKdenemerged from the infection of DEN NS1-expressing cells with YF $Delta$ SK.The appearance of this virus paralleled the growth of YF $Delta$ SK onthese cells, but at slightly lower titers. These data furthersupport the hypothesis that YF $Delta$ SK is incapable of utilizing DENNS1 for replication but that a subset of YF $Delta$ SK able to utilizeDEN NS1 can be selected by growth on DEN NS1-expressing cells.

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FIG. 4. Growth of YF $Delta$ SK on various cell populations. (A) BHK-SINrep21 cell monolayers (expressing YF NS1 [

], DEN NS1 [

], or GFP [ $black-lozenge$ ]) were infected with YF $Delta$ SK (MOI, 10) for 1 h, followed by three washes with PBS. At 12-h intervals, the growth media were removed and replaced with fresh media, clarified, and stored at $-$ 80°C. Virus titers were determined on YF NS1-expressing cells and plotted on a semilogarithmic scale. (B) The titers of the same samples from panel A determined on DEN NS1-expressing cells. The broken line indicates the detection limit of these plaque assays. The data represent the cumulative virus yields and are expressed as the means of the sum ± standard deviations for three independent experiments.

Isolation of YF $Delta$ SKden variants. In order to examine the genetic basis of the YF $Delta$ SKden phenotype, three YF $Delta$ SKden variants were independently derived from separatetransfections of YF $Delta$ SK RNA and isolated by two rounds of plaquepurification on DEN NS1-expressing cells. Two of these viruses,YF $Delta$ SKden 1.7 and YF $Delta$ SKden 2.5, were picked from medium-sized plaques,while a third virus, YF $Delta$ SKden 3.1, was a large-plaquevariant.

The growth characteristics of the isolated YF $Delta$ SKden variants were examined on both YF NS1- and DEN NS1-expressing cells. Allthree viruses replicated to similar levels on both cell types(Fig. 5A). This result confirmed the hypothesis that YF $Delta$ SKdencan infect either cell type and, therefore, that YF $Delta$ SKden is indeeda subset of YF $Delta$ SK. YF $Delta$ SKden 3.1 demonstrated a slightly higherlevel of growth at 24 h which may be related to its larger plaquesize. All viruses required the expression of NS1 in trans forgrowth (data not shown). Thus, these data demonstrate that thesethree virus isolates exhibit the YF $Delta$ SKden phenotype.

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FIG. 5. YF $Delta$ SKden can utilize DEN NS1 for RNA replication. (A) Growth analysis of independently derived YF $Delta$ SKden 1.7, 2.5, and 3.1. BHK-SINrep21 cells expressing YF NS1 (solid symbols) or DEN NS1 (open symbols) were infected with the indicated YF $Delta$ SKden isolates (MOI, 10) for 1 h, followed by three washes with PBS. Virus growth media were sampled at 0, 24, and 48 h postinfection, clarified, and stored at $-$ 80°C. Virus titers were determined on BHK-SINrep21/YF NS1 cells. The lower limit of the graph indicates the limit of detection in the plaque assays. (B) RNA replication of YF $Delta$ SKden. BHK-SINrep21 cells expressing YF NS1 (lanes 2 to 7), DEN NS1 (lanes 8 to 13), or GFP (lanes 14 to 19) were infected with the indicated viruses (MOI, 10). Total cellular RNAs were harvested at 16 h postinfection and subjected to RPA analysis of viral plus strands. MOCK, mock infection.

The RNA replication of YF $Delta$ SKden isolates was compared to that of YF 17D and YF $Delta$ SK on YF NS1-, DEN NS1-, and GFP-expressingcells by examination of the accumulation of viral plus strandsat 16 h postinfection by an RPA. Shown in Fig. 5B is a relativelylong exposure used in order to reveal any weak signals that mighthave been present. Plus strands were detected as a major 260-nucleotideband and a minor ~270-nucleotide band corresponding to a productof incomplete RNase digestion, as previously described (25).Abundant viral plus strands were specifically detected in allBHK-SINrep21/YF NS1 cells that were infected with a YF isolate(Fig. 5B, lanes 2 to 7). The requirement for NS1 expression byall YF $Delta$ SK derivatives was shown by the absence of any plus-strandsignal in cells expressing GFP (Fig. 5B, lanes 14 to 19). In DENNS1-expressing cells, only YF 17D and the three YF $Delta$ SKden isolatesdemonstrated plus-strand accumulation (Fig. 5B, lanes 9 and 11to 13). The parental virus, YF $Delta$ SK, failed to show evidence ofviral RNA replication on this cell type (Fig. 5B, lane 10). Whilequantitation standards were not analyzed in this experiment, therelative intensities of these bands reflect differences in RNAreplication rates over the first 16 h of infection. Notably, DENNS1 appeared to have a somewhat inhibitory effect on the replicationof YF 17D (see Discussion). Furthermore, YF $Delta$ SKden 3.1 replicatedto a higher level than the other YF $Delta$ SKden isolates on this celltype, consistent with the larger plaque size of this isolate.These data strongly indicate that the selected YF $Delta$ SKden isolatesare YF $Delta$ SK variants that have gained the capacity to utilize DENNS1 for the process of RNAreplication.

Genetic analysis of the YF $Delta$ SKden phenotype. Consensus sequences were determined for regions of the viral genomes by isolating virion RNAs and amplifying the regions byreverse transcriptase PCR. We hypothesized that NS1 would likelyinteract with a membrane-spanning viral NS protein, so we initiallyfocused our attention on the NS2A, NS4A, and NS4B regions of thegenomes as well as the residual NS1 gene. In sequencing approximately2.5 kb from each of the genomes, we found only a single pointmutation. Surprisingly, the same change was found in all threeindependently derived virus genomes, a point substitution at position5783, coding for a change of Asn to Tyr at codon 42 of the NS4Agene (Fig. 6). The sequence at this position of YF $Delta$ SK and theYF $Delta$ SKden derivatives was confirmed in multiple sequencing reactions.

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FIG. 6. Summary of YF $Delta$ SKden sequence analysis. Shown at the top is the YF $Delta$ SK genome. Thick bars below the genome indicate regions of the viral cDNAs that were sequenced. A single point substitution at position 5783, coding for a change of Asn (N) to Tyr (Y), is indicated.

In order to determine if the NS4A-N42Y change could confer the YF $Delta$ SKden phenotype, this single substitution was introducedinto pACNR/YF $Delta$ SK by site-directed mutagenesis. The infectivitiesof wild-type and mutant YF $Delta$ SK RNAs were measured by infectious-centerassays following RNA electroporation of cells expressing YF NS1or DEN NS1. The results of several experiments are summarizedin Fig. 7. Both types of RNAs were equally infectious in YF NS1-expressingcells, producing roughly 10⁶ PFU/µg of RNA transfected. In DEN NS1-expressing cells, wild-typeYF $Delta$ SK RNA had a low level of infectivity (~10³ PFU/µg). This result is consistent with the lack of replicationand de novo selection of additional variants, as described above.The NS4A-N42Y mutation conferred a wild-type level of infectivityto YF $Delta$ SK RNA in DEN NS1-expressing cells. Neither type of RNAwas infectious (<5 PFU/µg) in GFP-expressing cells (data not shown).These data indicated that a single point mutation within NS4Awas sufficient to confer the YF $Delta$ SKden phenotype.

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FIG. 7. NS4A-N42Y can confer the YF $Delta$ SKden phenotype. The specific infectivities of wild-type YF $Delta$ SK RNA (white bars) or mutant YF $Delta$ SK RNA (gray bars) were assayed by transfection of cells expressing YF NS1 (left bars) or DEN NS1 (right bars). Values represent the log geometric means ± standard deviations for four independent experiments.

To better define the requirements at this position, several additional substitutions were introduced into the NS4A gene andtested as described above. The results from a representative experimentare shown in Table 2. All RNAs were tested at least twice, withsimilar results. In order to determine if the coding change ofNS4A-N42Y rather than the local RNA secondary structure was responsible,a second NS4A-N42Y mutant was made. This mutant, NS4A-N42Y2, utilizeda different Tyr codon and included nine additional silent mutationsin the surrounding codons. These mutations gave rise to RNA thatwas as infectious as that resulting from the NS4A-N42Y change,formally demonstrating that the coding change of Asn to Tyr wasindeed responsible for the YF $Delta$ SKden phenotype. A variety of othersubstitutions were tolerated at this position by YF NS1, whileDEN NS1 seemed to exclude the uncharged polar residues Asn andGln but not Ser. NS4A-N42D, which substituted a carboxyl groupfor the terminal amide on Asn, produced a partial restorationof DEN NS1 function. Another residue that led to an intermediatephenotype was the moderately hydrophobic Met. Aromatic residuesat this position, as well as the cyclic basic residue His, wereall tolerated.

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TABLE 2. Effects of mutations at NS4A position 42

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The results presented here demonstrate that DEN NS1 is unable to trans complement YF $Delta$ SK due to its inability to participatein early RNA replication. Based on this system, YF $Delta$ SK variantsable to utilize DEN NS1 were selected, and genetic analysis ofthe adapted variants indicated that a single point substitutionin NS4A was sufficient to mediate this phenotype. These findingshave implications for understanding the role of NS1 in the replicationof viral RNA, a cytoplasmic process occurring at membraneinterfaces.

DEN NS1 does not function in YF RNA replication. Our initial stocks of YF $Delta$ SK did not grow or form plaques on DEN NS1-expressing cells, although efficient trans complementationwas demonstrated by YF NS1. Most significantly, there were undetectablelevels of RNA replication by this virus in DEN NS1-expressingcells. An inoculum of 10⁷ PFU must contain at least this number of genomes. Thus, we inferthat when ~10⁷ minus strands are detected in the samples during synchronizedinfection, the first minus strands are being synthesized. Thistime appeared to be shortly after 4 h postinfection of YF NS1-expressingcells with YF $Delta$ SK, consistent with our previous report (25).Note that this level of minus-strand accumulation was never detectedin YF $Delta$ SK-infected DEN NS1-expressing cells, indicating that RNAreplication was blocked prior to or at initial minus-strandsynthesis.

The patterns of DEN NS1 expression via the pSINrep21 vector closely resembled those of authentic DEN NS1 in cells infectedwith DEN-2. Furthermore, the levels of protein expression werecomparable to that produced by DEN-2-infected cells as well asto the levels of YF NS1 expression sufficient for complementationof YF $Delta$ SK. Thus, these considerations do not sufficiently explainthe inability of DEN NS1 to trans complement YF $Delta$ SK.

NS1 is among the more conserved of the flavivirus NS proteins. The NS1 proteins used in this study have 44% identity and 65%homology (PAM 250 index [12a]) at the amino acid level. Both Asn-linkedglycosylation sites and all 12 cysteine residues are conserved,suggesting conservation of structural features as well. Whileit has never been formally demonstrated that DEN and YF utilizetheir NS1 proteins for the same function(s), it seems unlikelythat a protein required for RNA replication would demonstratehigh functional divergence among closely related viruses. To addressthis point, as well as to examine the reciprocal trans complementationof DEN-2 with YF NS1, we constructed a deletion variant homologousto YF $Delta$ SK by using an infectious DEN-2 cDNA clone (a kind giftfrom Richard Kinney, Centers for Disease Control and Prevention).We were unable to demonstrate complementation of this genome (DEN $Delta$ SK)with either DEN NS1 or YF NS1 (data not shown), preventing directanalysis of these points. The inability of DEN NS1 to trans complementDEN $Delta$ SK could be due to differences in DEN-2 strains, since theNS1 gene was derived from DEN-2 strain PR-159(S1), while the infectiouscDNA was from DEN-2 strain 16681. Alternatively, the toleranceof DEN-2 for deletions in the NS1 gene may be different from thatof YF. Nevertheless, it appears that NS1 is required for DEN-2replication (23), and we look forward to understanding its rolein this viral system. Taken together, the above data indicatedthat NS1 functions in a flavivirus-specific manner and suggestedthat DEN NS1 does not productively interact with the YF replicationmachinery.

Genetic screen for YF $Delta$ SKden variants. In order to define such an interaction, we selected for YF $Delta$ SKden variants able to utilize DEN NS1. Because the NS1 gene hasbeen deleted from YF $Delta$ SK and was supplied in trans, such variantswere likely to contain suppressor mutations with the potentialto reveal other viral genes involved in the function of NS1. Asin all genetic selections, the ability to select a given phenotypeis dependent on the genetic heterogeneity present in the initialpopulation. To facilitate this selection, we capitalized on theimproved specific infectivity of transcripts derived from pACNR/YF $Delta$ SKin order to explore variant YF $Delta$ SK genomes. In this regard, itmay be instructive to consider the potential sources of adaptivemutations.

Given that YF $Delta$ SK demonstrated undetectable RNA replication on DEN NS1-expressing cells (Fig. 2B), the possibility that adaptivemutations existed in the population of input RNA molecules thatwere used for transfection must be considered. The fidelity ofSP6 RNA polymerase has not been reported; however, the relatedenzyme from bacteriophage T7 has an estimated error frequencyof 10⁴ (3, 44). Thus, for a genome the size of YF $Delta$ SK (~10 kb),RNA transcripts containing single point mutations are expectedto be as abundant as the wild type, each about 37% of the RNApopulation. One microgram of this transcript should contain approximately2 × 10⁶ copies of YF $Delta$ SK with the single point mutation A5783T. However,the actual misincorporation rate at any given position is likelyto be influenced by other factors specific for the polymeraseand the local template structure. This might explain why Tyr seemedto be preferred although several other substitutions were foundto work in this position. Furthermore, our ability to sample anRNA population is limited by the efficiency with which transfectedRNAs initiate a productive infection. For reasons that remainobscure, only a small fraction of RNA transcripts actually yieldedplaque-forming units, ~10⁶ PFU/µg, which represents an RNA transfection efficiency of ~10⁵ PFU/RNA molecule. The latter point may help to explain why weinitially saw no sign of trans complementation of our originalYF $Delta$ SK stock on DEN NS1-expressing cells. Recall that this viruswas generated via the two-plasmid YF infectious clone and wasinitiated at a specific infectivity of 7 × 10² PFU/µg (25). Thus, this virus stock is likely to contain lessgenetic diversity initially due to this lower sampling rate. Basedon these considerations, it is clear that the process of RNA transcriptionmay produce sufficient genetic diversity to examine the constellationof YF $Delta$ SK single-point mutations but that this examination is subjectto the RNA samplingrate.

Another potential source of adaptive mutations was misincorporation by the YF replicase itself. Although YF replicase hasan unknown fidelity, studies of other RNA viruses indicate errorrates on the order of 10³ to 10⁴ (45, 47). Thus, one would expect YF $Delta$ SKden variants to arisenaturally in a population of YF $Delta$ SK isolates replicating in YFNS1-expressing cells. Indeed, passage of YF $Delta$ SK on DEN NS1-expressingcells selected for rare variants in a population of YF $Delta$ SK isolates(Fig. 4). However, it is unknown whether these variants existedin the RNA population used to derive the YF $Delta$ SK stock or whetherthey arose during virus passage. To address this question moredirectly, two YF $Delta$ SK isolates were independently derived by RNAtransfection and isolated by plaque purification on YF NS1-expressingcells (data not shown). YF $Delta$ SKden variants arose spontaneouslyafter passage of these virus stocks several times on YF NS1-expressingcells (data not shown), suggesting that adaptive mutations couldhave arisen during the process of YF RNA replication. These resultsmay also explain the absence of the YF $Delta$ SKden phenotype in ouroriginal YF $Delta$ SK stock (Fig. 1 and 2), which was passaged once followingtransfection and was therefore the product of a small (albeitunknown) number of RNA replicationcycles.

YF $Delta$ SKden isolates are variants of YF $Delta$ SK able to utilize DEN NS1. Given the above arguments for the generation of genetic diversity in RNA virus populations, several lines of evidence supportthe hypothesis that YF $Delta$ SKden isolates are variants of YF $Delta$ SK ableto utilize DEN NS1. Only a small fraction of YF $Delta$ SK RNA transfectedinto DEN NS1-expressing cells was infectious, yielding plaqueswith a variety of sizes and morphologies. Unlike YF $Delta$ SK initiatedon YF NS1-expressing cells, DEN NS1-initiated virus demonstratedthe ability to form plaques on both cell types. Similarly, YF $Delta$ SKdenisolates could also be derived by passage of YF $Delta$ SK on cells expressingDEN NS1 but not on cells expressing YF NS1. The lag that was observedin the growth of YF $Delta$ SK was consistent with the emergence of asubpopulation with the ability to replicate in DEN NS1-expressingcells. Furthermore, YF $Delta$ SKden isolates obtained by plaque purificationwere able to grow on both cell types and demonstrated the abilityto replicate their viral RNA on DEN NS1-expressing cells. Thelack of detectable viruses with the YF $Delta$ SKden phenotype in YF NS1-initiatedvirus populations (<5 PFU/ml) may suggest that YF $Delta$ SKden is ata selective disadvantage for growth in YF NS1-expressing cellswhen coinfected with YF $Delta$ SK. Taken together, these data argue thatYF $Delta$ SKden isolates, unlike the larger YF $Delta$ SK population, were ableto utilize DEN NS1 for RNA replication andgrowth.

It was remarkable that only a single substitution, NS4A-N42Y, was identified multiple times by sequencing of the isolatedYF $Delta$ SKden genomes. While it is entirely possible that other adaptivemutations exist in YF $Delta$ SKden populations, we have not yet observedother sequence changes. Nevertheless, this single mutation wassufficient to confer high infectivity to YF $Delta$ SK RNA in DEN NS1-expressingcells. We may conclude that NS4A-N42Y is sufficient to mediatethis phenotype, although this particular change may not be necessary.In this regard, several additional substitutions were tested andalso found to permit mutant YF $Delta$ SK genomes to utilize DEN NS1.Of the amino acids tested, the only ones that were not toleratedby DEN NS1 were Asn and Gln, while Asp and Met gave intermediatephenotypes. Thus, the rules of amino acid substitution at thisposition for DEN NS1 utilization are not yet clear. However, theseresults support the hypothesis that a genetic interaction existsbetween NS1 and NS4A. Note that the type of genetic interactionthat we are discussing here does not necessarily imply a directprotein-protein interaction of NS1 and NS4A gene products. Becausethe general features of flavivirus RNA replication appear to beconserved across the genus (11, 12, 21), these findingsmay extend to other flaviviruses, although this awaits experimentalproof.

In addition to the complementation of YF $Delta$ SKden, DEN NS1 had an inhibitory effect on wild-type YF 17D, which was seen as reducedlevels of viral plus-strand accumulation (Fig. 5B, lanes 9 and15). Inhibition of YF 17D replication was also evident as a reproducible1- to 2-log₁₀ decrease in viral titers during single-cycle growthexperiments (data not shown). This result is in contrast to aslight increase in YF 17D replication with the expression of YFNS1 (Fig. 5B, lanes 3 and 15; see also Fig. 5, 6, and 7 in reference25). To determine if this inhibition could be mediated by adominant-negative effect of DEN NS1, perhaps through the usurpingof NS4A, we introduced the NS4A-N42Y mutation into the wild-typeYF 17D genome. The resultant viruses did not, however, overcomethe inhibitory effect of DEN NS1 (data not shown), suggestingthat other mechanisms may also be involved. For instance, YF NS1and DEN NS1 may form inactive heterodimers. As mentioned above,YF $Delta$ SKden 3.1 seemed to have an enhanced capacity for replicationin DEN NS1-expressing cells (see, for instance, Fig. 5B, lanes11, 12, and 13). This virus is likely to contain, in additionto NS4A-N42Y, adaptive mutations which may overcome this inhibition.Therefore, further characterization of this virus is underway.

Prospects for understanding replicase ultrastructure. It is interesting that an adaptive mutation was mapped to NS4A. The product of this gene, a small hydrophobic protein, hasan unknown function in the life cycle of flaviviruses. Althoughrecent results suggest that NS4A is associated with flavivirusreplicase components (27), our results provide the first geneticdata indicating that NS4A is involved in the process of RNA replication.NS4A is produced from the viral polyprotein via cleavage at itsN and C termini by the viral serine protease (Fig. 8A). Both cleavageevents appear to be delayed or regulated, since the putative NS4Aprecursors NS3-4A and NS4A-4B have been identified in flavivirus-infectedcells (7, 33). Protease cleavage of NS4A-B appears to coordinatea downstream cleavage event for signal peptidase, which generatesa small "2K" signal peptide and the N terminus of NS4B (24,32). This coordinated cleavage may represent a mechanism forthe regulation of replicase function by the viral protease, perhapsanalogous to the switch from minus-strand to plus-strand synthesismediated by the alphavirus cysteine protease (22, 41). Becauselittle is known about the importance of NS4A-processing events,further investigation will be required to understand the relevantcontext in which the NS4A-N42Y mutation functions.

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FIG. 8. Model of NS4A topology and secondary structure. (A) The topology of NS4A/2K was modeled as described in Materials and Methods. The arrows, open box, and black dot indicate viral serine protease cleavage sites, a signal peptidase cleavage site, and the approximate location of NS4A residue 42, respectively. (B) Several flavivirus NS4A coding regions were aligned with YF NS4A residues 11 to 60. The virus sequences shown (and their GenBank accession numbers) are as follows: YF 17D (P03314), DEN-1 (P33478), DEN-2 (P123823), DEN-3 (P27915), DEN-4 (P09866), Japanese encephalitis (JE) (P32886), Kunjin (KUN) (P14335), tick-borne encephalitis (TBE) (P14336), and West Nile (WN) (P06935). Shown below the alignment is a prediction of the secondary structure: H, helix; L, loop; E, strand; dot, not predictable. Also shown is the beginning of the first putative transmembrane domain, depicted as a box. The location of YF NS4A residue 42 is indicated above the alignment by a black dot.

Genetic interaction between NS1 and NS4A helps to resolve an important topological issue, namely, how a protein in the secretorypathway can be required for RNA replication, a process that occursin the cytoplasm of infected cells in close association with virus-inducedmembrane structures. The two major enzymatic components of thereplicase, NS3 and NS5, are predicted to reside in the cytoplasm(34). In support of this model, both were shown to be sensitiveto trypsin digestion in extracts made from infected cells in theabsence of detergents (5). The interaction of NS1 and cellularmembranes remains more complex, although several lines of evidenceindicate that NS1 resides in the luminal side of an extracytoplasmiccompartment. As mentioned earlier, processing at the N and C terminiof NS1 is mediated by enzymes in the ER; NS1 is glycosylated anddisulfide bonded, and a portion of it is secreted. All of theseprocesses indicate that NS1 forms in the secretory pathway. Shortlyafter synthesis, NS1 acquires hydrophobic properties and associateswith membranes (51); these steps may correlate with the formationof NS1 homodimers (52). NS1 does not contain any putative transmembranedomains (36) or known posttranslational lipid modifications.Mutagenesis of the first glycosylation site of YF NS1 demonstratedthat this modification is important for efficient RNA replication(29), indicating that NS1 requires translocation into the ERfor function. We have recently expressed a version of NS1 lackingits signal sequence and found that it does not function in transcomplementation (28). Furthermore, resistance to trypsin inthe absence of detergents largely supports the extracytoplasmicsequestration of NS1, although a proportion of NS1 was sensitiveto this treatment (5). However, these authors did not excludethe possible disruption of an NS1-containing compartment duringthe extraction procedure, which may explain this partial sensitivity.Taken together, these data indicate that NS1 is in a compartmenttopologically distinct from the cytoplasm, where the process ofRNA replicationoccurs.

NS4A is predicted to be membrane spanning (34), although biochemical data on the topology of this protein are lacking. Wehave modeled the secondary structure of this protein and its interactionwith cellular membranes by using current predictive algorithmsas described in Materials and Methods. The N and C termini ofNS4A are expected to be cytoplasmic, consistent with their generationby the viral serine protease (Fig. 8A). The N-terminal regionof NS4A (YF 17D codons 2108 to 2160) is predicted to be cytoplasmicand possibly rich in alpha helices and to be followed by two transmembranedomains separated by a short peptide (YF 17D codons 2161 to 2178,2179 to 2194, and 2195 to 2219) and a short C-terminal domain(YF 17D codons 2220 to 2233). The NS4A-N42Y mutation localizesto a putative alpha-helical region in the cytoplasmic N-terminaldomain, an observation that is inconsistent with this residuebeing involved in a direct protein-protein interaction with NS1.Perhaps the N-terminal region of NS4A affects the structure ofthe luminal peptide, which might interact with NS1. Alternatively,an interaction between NS1 and the luminal peptide might inducea conformational effect on this region of NS4A, allowing it torecruit cytoplasmic replicase components. As noted above, thegenetic interaction between NS1 and NS4A does not exclude theinvolvement of other replicase components, and we do not meanto necessarily imply a direct protein-protein interaction. Froman alignment of several flavivirus NS4A genes, it is apparentthat a His residue is conserved at this position between DEN isotypes,while Met is preferred at NS4A position 42 in tick-borne and othermosquito-borne flaviviruses (Fig. 8B). Clearly, more work needsto be done to examine the structure and function of this regionof NS4A in order to determine the basis for our genetic observations.Nevertheless, the involvement of NS4A, a putative transmembraneprotein, in NS1 utilization may provide a solution to the puzzleof NS1 versus replicasetopology.

Cytological studies of the flavivirus replicase have indicated that NS1 and NS4A can both be localized to perinuclear clustersof vesicles bound by a larger membrane, termed vesicle packets(26, 27, 50). It is unclear whether this larger membrane,which appears to be contiguous with the ER, represents an enclosedvesicle or a transverse slice of a membranous pocket. An indicationthat vesicle packets are associated with replication has beenprovided by labeling studies with an antiserum that recognizesdouble-stranded RNA. NS2A and NS3 are also associated with thesestructures, while other NS proteins have been excluded (27,50). In addition to vesicle packets, NS4A localizes to othervirus-induced membrane structures, termed convoluted membranesor paracrystalline arrays. The role of these structures in infectedcells is unclear, although it has been suggested that they representsites of polyprotein processing (50). The colocalization ofNS1, NS4A, and a marker of RNA replication in vesicle packetssupports our genetic data indicating that an NS1-NS4A interactionis important in the process of RNAreplication.

Biochemical studies have also indicated that NS4A interacts with other replicase components. Both NS1 and NS4A appear to cosedimentwith dense membrane fractions enriched in RNA-dependent RNA polymeraseactivity (10). Furthermore, it was recently reported that afusion protein of NS4A and glutathione-S-transferase could retainseveral virus-specific proteins on glutathione beads, includingNS1, NS2A, NS3, NS3-4A, NS4A, and NS5 (27). The binding of NS2Aand NS3-4A appears to be sensitive to RNase treatment, suggestingthat an indirect interaction is involved. The involvement of bothNS1 and NS4A in these complexes further supports a model of theirinteraction.

Our approach to understanding the flavivirus replicase has been to use genetic means. A particularly useful technique hasbeen the trans complementation of NS proteins, which previouslyrevealed a requirement for NS1 in early RNA replication (25).We have now extended our studies to demonstrate a genetic interactionbetween NS1 and NS4A. It was recently reported that a Kunjin virusgenome bearing lethal mutations in the RNA polymerase or putativemethyltransferase domains of NS5 could also be complemented intrans by use of a Kunjin virus replicon lacking structural genes(20). This approach shows promise for demonstrating the transcomplementation of multiple NS genes. However, this system differsfrom ours in at least two respects. It appears that a significantamount of Kunjin virus replicon is packaged in trans, eliminatingthe ability to examine helper-free mutant virus stocks. Furthermore,the expression of the complementing NS protein is coupled to itsfunction, preventing the future application of this system tothe probing of NS protein structure and function. We have usedour system, which circumvents both of these disadvantages, toreveal the functional roles of flavivirusNS1.

Future directions. This study reveals a genetic interaction between NS1 and NS4A and demonstrates the significance of this interaction for RNAreplication. Further studies are needed to directly examine thenature of this interaction and of other proteins in the replicase.The integration of biochemical, structural, and genetic approachesshows great promise in unraveling the intricacies of flavivirusreplicase structure and function. Here we have demonstrated atool that we expect will be useful in thisendeavor.

	ACKNOWLEDGMENTS

We thank Rebecca Moran for expert technical assistance. We are also grateful to many colleagues for helpful discussions duringthe course of this work and to Sean Amberg, Richard Hardy, andMara Lippa for critical reading of themanuscript.

This work was supported in part by a grant from the Public Health Service(AI31501).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Molecular Microbiology, Washington University School of Medicine, 660S. Euclid Ave., St. Louis, MO 63110-1093. Phone: (314) 362-2842.Fax: (314) 362-1232. E-mail: rice{at}borcim.wustl.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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2. Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1993. Current protocols in molecular biology. Greene Publishing Associates, New York, N.Y.

3. Boyer, J. C., K. Bebenek, and T. A. Kunkel. 1992. Unequal human immunodeficiency virus type 1 reverse transcriptase error rates with RNA and DNA templates. Proc. Natl. Acad. Sci. USA 89:6919-6923[Abstract/Free Full Text].

4. Bredenbeek, P. J., E. Kooi, B. D. Lindenbach, M. Lucassen, N. Huijkman, W. J. M. Spaan, and C. M. Rice. 1999. Unpublished data.

5. Cauchi, M. R., E. A. Henchal, and P. J. Wright. 1991. The sensitivity of cell-associated dengue virus proteins to trypsin and the detection of trypsin-resistant fragments of the nonstructural glycoprotein NS1. Virology 180:659-667[Medline].

6. Chambers, T. J., C. S. Hahn, R. Galler, and C. M. Rice. 1990. Flavivirus genome organization, expression, and replication. Annu. Rev. Microbiol. 44:649-688[Medline].

7. Chambers, T. J., D. W. McCourt, and C. M. Rice. 1990. Production of yellow fever virus proteins in infected cells: identification of discrete polyprotein species and analysis of cleavage kinetics using region-specific polyclonal antisera. Virology 177:159-174[Medline].

8. Chambers, T. J., D. W. McCourt, and C. M. Rice. 1989. Yellow fever virus proteins NS2A, NS2B, and NS4B: identification and partial N-terminal amino acid sequence analysis. Virology 169:100-109[Medline].

9. Chambers, T. J., R. C. Weir, A. Grakoui, D. W. McCourt, J. F. Bazan, R. J. Fletterick, and C. M. Rice. 1990. Evidence that the N-terminal domain of nonstructural protein NS3 from yellow fever virus is a serine protease responsible for site-specific cleavages in the viral polyprotein. Proc. Natl. Acad. Sci. USA 87:8898-8902[Abstract/Free Full Text].

10. Chu, P. W., and E. G. Westaway. 1992. Molecular and ultrastructural analysis of heavy membrane fractions associated with the replication of Kunjin virus RNA. Arch. Virol. 125:177-191[Medline].

11. Chu, P. W. G., and E. G. Westaway. 1985. Replication strategy of Kunjin virus: Evidence for recycling role of replicative form RNA as template in semiconservative and asymmetric replication. Virology 140:68-79[Medline].

12. Cleaves, G. R., T. E. Ryan, and R. W. Schlesinger. 1981. Identification and characterization of type 2 dengue virus replicative intermediate and replicative form RNAs. Virology 111:73-83[Medline].

12a. Dayhoff, M. O., R. M. Schwartz, and B. C. Orcott. 1978. A model of evolutionary change in proteins, p. 345-352. In M. O. Dayhoff (ed.), Atlas of protein sequence and structure, vol. 5. National Biomedical Research Foundation, Silver Spring, Md.

13. Falgout, B., R. Chanock, and C. J. Lai. 1989. Proper processing of dengue virus nonstructural glycoprotein NS1 requires the N-terminal hydrophobic signal sequence and the downstream nonstructural protein NS2A. J. Virol. 63:1852-1860[Abstract/Free Full Text].

14. Falgout, B., and L. Markoff. 1995. Evidence that flavivirus NS1-NS2A cleavage is mediated by a membrane-bound host protease in the endoplasmic reticulum. J. Virol. 69:7232-7243[Abstract].

15. Gorbalenya, A. E., A. P. Donchenko, E. V. Koonin, and V. M. Blinov. 1989. N-terminal domains of putative helicases of flavi- and pestiviruses may be serine proteases. Nucleic Acids Res. 17:3889-3897[Abstract/Free Full Text].

16. Gorbalenya, A. E., E. V. Koonin, A. P. Donchenko, and V. M. Blinov. 1989. Two related superfamilies of putative helicases involved in replication, recombination, repair and expression of DNA and RNA genomes. Nucleic Acids Res. 17:4713-4729[Abstract/Free Full Text].

17. Grun, J. B., and M. A. Brinton. 1988. Separation of functional West Nile virus replication complexes from intracellular membrane fragments. J. Gen. Virol. 69:3121-3127[Abstract/Free Full Text].

18. Hope, D. A., S. E. Diamond, and K. Kirkegaard. 1997. Genetic dissection of interaction between poliovirus 3D polymerase and viral protein 3AB. J. Virol. 71:9490-9498[Abstract].

19. Kao, C. C., and P. Ahlquist. 1992. Identification of the domains required for direct interaction of the helicase-like and polymerase-like RNA replication proteins of brome mosaic virus. J. Virol. 66:7293-7302[Abstract/Free Full Text].

20. Khromykh, A. A., M. T. Kenney, and E. G. Westaway. 1998. trans-Complementation of flavivirus RNA polymerase gene NS5 by using Kunjin virus replicon-expressing BHK cells. J. Virol. 72:7270-7279[Abstract/Free Full Text].

21. Lancaster, M. U., S. I. Hodgetts, J. S. Mackenzie, and N. Urosevic. 1998. Characterization of defective viral RNA produced during persistent infection of Vero cells with Murray Valley encephalitis virus. J. Virol. 72:2474-2482[Abstract/Free Full Text].

22. Lemm, J. A., T. Rumenapf, E. G. Strauss, J. H. Strauss, and C. M. Rice. 1994. Polypeptide requirements for assembly of functional Sindbis virus replication complexes: a model for the temporal regulation of minus- and plus-strand RNA synthesis. EMBO J. 13:2925-2934[Medline].

23. Levis, R. Personal communication.

24. Lin, C., S. M. Amberg, T. J. Chambers, and C. M. Rice. 1993. Cleavage at a novel site in the NS4A region by the yellow fever virus NS2B-3 proteinase is a prerequisite for processing at the downstream 4A/4B signalase site. J. Virol. 67:2327-2335[Abstract/Free Full Text].

25. Lindenbach, B. D., and C. M. Rice. 1997. trans-Complementation of yellow fever virus NS1 reveals a role in early RNA replication. J. Virol. 71:9608-9617[Abstract].

26. Mackenzie, J. M., M. K. Jones, and P. R. Young. 1996. Immunolocalization of the dengue virus nonstructural glycoprotein NS1 suggests a role in viral RNA replication. Virology 220:232-240[Medline].

27. Mackenzie, J. M., A. A. Khromykh, M. K. Jones, and E. G. Westaway. 1998. Subcellular localization and some biochemical properties of the flavivirus Kunjin nonstructural proteins NS2A and NS4A. Virology 245:203-215[Medline].

28. Moorman, N., B. D. Lindenbach, and C. M. Rice. Unpublished data.

29. Muylaert, I. R., T. J. Chambers, R. Galler, and C. M. Rice. 1996. Mutagenesis of the N-linked glycosylation sites of the yellow fever virus NS1 protein: effects on virus replication and mouse neurovirulence. Virology 222:159-168[Medline].

30. Muylaert, I. R., R. Galler, and C. M. Rice. 1997. Genetic analysis of the yellow fever virus NS1 protein: identification of a temperature-sensitive mutation which blocks RNA accumulation. J. Virol. 71:291-298[Abstract].

31. Novak, J. E., and K. Kirkegaard. 1991. Improved method for detecting poliovirus negative strands used to demonstrate specificity of positive-strand encapsidation and the ratio of positive to negative strands in infected cells. J. Virol. 65:3384-3387[Abstract/Free Full Text].

32. Preugschat, F., and J. H. Strauss. 1991. Processing of nonstructural proteins NS4A and NS4B of dengue 2 virus in vitro and in vivo. Virology 185:689-697[Medline].

33. Preugschat, F., C.-W. Yao, and J. H. Strauss. 1990. In vitro processing of dengue virus type 2 nonstructural proteins NS2A, NS2B, and NS3. J. Virol. 64:4364-4374[Abstract/Free Full Text].

34. 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. Raven Press, New York, N.Y.

35. Rice, C. M., A. Grakoui, R. Galler, and T. J. Chambers. 1989. Transcription of infectious yellow fever virus RNA from full-length cDNA templates produced by in vitro ligation. New Biol. 1:285-296[Medline].

36. Rice, C. M., E. M. Lenches, S. R. Eddy, S. J. Shin, R. L. Sheets, and J. H. Strauss. 1985. Nucleotide sequence of yellow fever virus: implications for flavivirus gene expression and evolution. Science 229:726-733[Abstract/Free Full Text].

37. Rost, B., and C. Sander. 1994. Combining evolutionary information and neural networks to predict protein secondary structure. Proteins 19:55-72[Medline].

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41. Shirako, Y., and J. H. Strauss. 1994. Regulation of Sindbis virus RNA replication: Uncleaved P123 and nsP4 function in minus-strand RNA synthesis, whereas cleaved products from P123 are required for efficient plus-strand RNA synthesis. J. Virol. 185:1874-1885.

42. Smith, G. W., and P. J. Wright. 1985. Synthesis of proteins and glycoproteins in dengue type 2 virus-infected Vero and Aedes albopictus cells. J. Gen. Virol. 66:559-571[Abstract/Free Full Text].

43. Sonnhammer, E. L., S. R. Eddy, E. Birney, A. Bateman, and R. Durbin. 1998. Pfam: multiple sequence alignments and HMM-profiles of protein domains. Nucleic Acids Res. 26:320-322[Abstract/Free Full Text].

44. Sooknanan, R., M. Howes, L. Read, and L. T. Malek. 1994. Fidelity of nucleic acid amplification with an avian myeloblastosis virus reverse transcriptase and T7 RNA polymerase. BioTechniques 17:1077-1085[Medline].

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46. Tan, B. H., J. Fu, R. J. Sugrue, E. H. Yap, Y. C. Chan, and Y. H. Tan. 1996. Recombinant dengue type 1 virus NS5 protein expressed in Escherichia coli exhibits RNA-dependent RNA polymerase activity. Virology 216:317-325[Medline].

47. Ward, C. D., and J. B. Flanegan. 1988. Direct measurement of the poliovirus RNA polymerase error frequency in vitro. J. Virol. 62:558-562[Abstract/Free Full Text].

48. Wengler, G., and G. Wengler. 1991. The carboxy-terminal part of the NS3 protein of the West Nile flavivirus can be isolated as a soluble protein after proteolytic cleavage and represents an RNA-stimulated NTPase. Virology 184:707-715[Medline].

49. Wengler, G., and G. Wengler. 1993. The NS3 nonstructural protein of flaviviruses contains an RNA triphosphatase activity. Virology 197:265-273[Medline].

50. Westaway, E. G., J. M. Mackenzie, M. T. Kenney, M. K. Jones, and A. A. Khromykh. 1997. Ultrastructure of Kunjin virus-infected cells: colocalization of NS1 and NS3 with double-stranded RNA and of NS2B with NS3 in virus-induced membrane structures. J. Virol. 71:6650-6661[Abstract].

51. Winkler, G., S. E. Maxwell, C. Ruemmler, and V. Stollar. 1989. Newly synthesized dengue-2 virus nonstructural protein NS1 is a soluble protein but becomes partially hydrophobic and membrane-associated after dimerization. Virology 171:302-305[Medline].

52. Winkler, G., V. B. Randolph, G. R. Cleaves, T. E. Ryan, and V. Stollar. 1988. Evidence that the mature form of the flavivirus nonstructural protein NS1 is a dimer. Virology 162:187-196[Medline].

53. Xiang, W., A. Cuconati, D. Hope, K. Kirkegaard, and E. Wimmer. 1998. Complete protein linkage map of poliovirus P3 proteins: interaction of polymerase 3Dpol with VPg and with genetic variants of 3AB. J. Virol. 72:6732-6741[Abstract/Free Full Text].

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1.	Agapov, E. V., I. Frolov, B. D. Lindenbach, B. M. Prágai, S. Schlesinger, and C. M. Rice. 1998. Noncytopathic Sindbis virus RNA vectors for heterologous gene expression. Proc. Natl. Acad. Sci. USA 95:12989-12994[Abstract/Free Full Text].
2.	Ausubel, F. M., R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.). 1993. Current protocols in molecular biology. Greene Publishing Associates, New York, N.Y.
3.	Boyer, J. C., K. Bebenek, and T. A. Kunkel. 1992. Unequal human immunodeficiency virus type 1 reverse transcriptase error rates with RNA and DNA templates. Proc. Natl. Acad. Sci. USA 89:6919-6923[Abstract/Free Full Text].
4.	Bredenbeek, P. J., E. Kooi, B. D. Lindenbach, M. Lucassen, N. Huijkman, W. J. M. Spaan, and C. M. Rice. 1999. Unpublished data.
5.	Cauchi, M. R., E. A. Henchal, and P. J. Wright. 1991. The sensitivity of cell-associated dengue virus proteins to trypsin and the detection of trypsin-resistant fragments of the nonstructural glycoprotein NS1. Virology 180:659-667[Medline].
6.	Chambers, T. J., C. S. Hahn, R. Galler, and C. M. Rice. 1990. Flavivirus genome organization, expression, and replication. Annu. Rev. Microbiol. 44:649-688[Medline].
7.	Chambers, T. J., D. W. McCourt, and C. M. Rice. 1990. Production of yellow fever virus proteins in infected cells: identification of discrete polyprotein species and analysis of cleavage kinetics using region-specific polyclonal antisera. Virology 177:159-174[Medline].
8.	Chambers, T. J., D. W. McCourt, and C. M. Rice. 1989. Yellow fever virus proteins NS2A, NS2B, and NS4B: identification and partial N-terminal amino acid sequence analysis. Virology 169:100-109[Medline].
9.	Chambers, T. J., R. C. Weir, A. Grakoui, D. W. McCourt, J. F. Bazan, R. J. Fletterick, and C. M. Rice. 1990. Evidence that the N-terminal domain of nonstructural protein NS3 from yellow fever virus is a serine protease responsible for site-specific cleavages in the viral polyprotein. Proc. Natl. Acad. Sci. USA 87:8898-8902[Abstract/Free Full Text].
10.	Chu, P. W., and E. G. Westaway. 1992. Molecular and ultrastructural analysis of heavy membrane fractions associated with the replication of Kunjin virus RNA. Arch. Virol. 125:177-191[Medline].
11.	Chu, P. W. G., and E. G. Westaway. 1985. Replication strategy of Kunjin virus: Evidence for recycling role of replicative form RNA as template in semiconservative and asymmetric replication. Virology 140:68-79[Medline].
12.	Cleaves, G. R., T. E. Ryan, and R. W. Schlesinger. 1981. Identification and characterization of type 2 dengue virus replicative intermediate and replicative form RNAs. Virology 111:73-83[Medline].
12a.	Dayhoff, M. O., R. M. Schwartz, and B. C. Orcott. 1978. A model of evolutionary change in proteins, p. 345-352. In M. O. Dayhoff (ed.), Atlas of protein sequence and structure, vol. 5. National Biomedical Research Foundation, Silver Spring, Md.
13.	Falgout, B., R. Chanock, and C. J. Lai. 1989. Proper processing of dengue virus nonstructural glycoprotein NS1 requires the N-terminal hydrophobic signal sequence and the downstream nonstructural protein NS2A. J. Virol. 63:1852-1860[Abstract/Free Full Text].
14.	Falgout, B., and L. Markoff. 1995. Evidence that flavivirus NS1-NS2A cleavage is mediated by a membrane-bound host protease in the endoplasmic reticulum. J. Virol. 69:7232-7243[Abstract].
15.	Gorbalenya, A. E., A. P. Donchenko, E. V. Koonin, and V. M. Blinov. 1989. N-terminal domains of putative helicases of flavi- and pestiviruses may be serine proteases. Nucleic Acids Res. 17:3889-3897[Abstract/Free Full Text].
16.	Gorbalenya, A. E., E. V. Koonin, A. P. Donchenko, and V. M. Blinov. 1989. Two related superfamilies of putative helicases involved in replication, recombination, repair and expression of DNA and RNA genomes. Nucleic Acids Res. 17:4713-4729[Abstract/Free Full Text].
17.	Grun, J. B., and M. A. Brinton. 1988. Separation of functional West Nile virus replication complexes from intracellular membrane fragments. J. Gen. Virol. 69:3121-3127[Abstract/Free Full Text].
18.	Hope, D. A., S. E. Diamond, and K. Kirkegaard. 1997. Genetic dissection of interaction between poliovirus 3D polymerase and viral protein 3AB. J. Virol. 71:9490-9498[Abstract].
19.	Kao, C. C., and P. Ahlquist. 1992. Identification of the domains required for direct interaction of the helicase-like and polymerase-like RNA replication proteins of brome mosaic virus. J. Virol. 66:7293-7302[Abstract/Free Full Text].
20.	Khromykh, A. A., M. T. Kenney, and E. G. Westaway. 1998. trans-Complementation of flavivirus RNA polymerase gene NS5 by using Kunjin virus replicon-expressing BHK cells. J. Virol. 72:7270-7279[Abstract/Free Full Text].
21.	Lancaster, M. U., S. I. Hodgetts, J. S. Mackenzie, and N. Urosevic. 1998. Characterization of defective viral RNA produced during persistent infection of Vero cells with Murray Valley encephalitis virus. J. Virol. 72:2474-2482[Abstract/Free Full Text].
22.	Lemm, J. A., T. Rumenapf, E. G. Strauss, J. H. Strauss, and C. M. Rice. 1994. Polypeptide requirements for assembly of functional Sindbis virus replication complexes: a model for the temporal regulation of minus- and plus-strand RNA synthesis. EMBO J. 13:2925-2934[Medline].
23.	Levis, R. Personal communication.
24.	Lin, C., S. M. Amberg, T. J. Chambers, and C. M. Rice. 1993. Cleavage at a novel site in the NS4A region by the yellow fever virus NS2B-3 proteinase is a prerequisite for processing at the downstream 4A/4B signalase site. J. Virol. 67:2327-2335[Abstract/Free Full Text].
25.	Lindenbach, B. D., and C. M. Rice. 1997. trans-Complementation of yellow fever virus NS1 reveals a role in early RNA replication. J. Virol. 71:9608-9617[Abstract].
26.	Mackenzie, J. M., M. K. Jones, and P. R. Young. 1996. Immunolocalization of the dengue virus nonstructural glycoprotein NS1 suggests a role in viral RNA replication. Virology 220:232-240[Medline].
27.	Mackenzie, J. M., A. A. Khromykh, M. K. Jones, and E. G. Westaway. 1998. Subcellular localization and some biochemical properties of the flavivirus Kunjin nonstructural proteins NS2A and NS4A. Virology 245:203-215[Medline].
28.	Moorman, N., B. D. Lindenbach, and C. M. Rice. Unpublished data.
29.	Muylaert, I. R., T. J. Chambers, R. Galler, and C. M. Rice. 1996. Mutagenesis of the N-linked glycosylation sites of the yellow fever virus NS1 protein: effects on virus replication and mouse neurovirulence. Virology 222:159-168[Medline].
30.	Muylaert, I. R., R. Galler, and C. M. Rice. 1997. Genetic analysis of the yellow fever virus NS1 protein: identification of a temperature-sensitive mutation which blocks RNA accumulation. J. Virol. 71:291-298[Abstract].
31.	Novak, J. E., and K. Kirkegaard. 1991. Improved method for detecting poliovirus negative strands used to demonstrate specificity of positive-strand encapsidation and the ratio of positive to negative strands in infected cells. J. Virol. 65:3384-3387[Abstract/Free Full Text].
32.	Preugschat, F., and J. H. Strauss. 1991. Processing of nonstructural proteins NS4A and NS4B of dengue 2 virus in vitro and in vivo. Virology 185:689-697[Medline].
33.	Preugschat, F., C.-W. Yao, and J. H. Strauss. 1990. In vitro processing of dengue virus type 2 nonstructural proteins NS2A, NS2B, and NS3. J. Virol. 64:4364-4374[Abstract/Free Full Text].
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