Nucleic Acid-Dependent Cross-Linking of the Nucleocapsid Protein of Sindbis Virus

doi:10.1128/JVI.74.9.4302-4309.2000

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Journal of Virology, May 2000, p. 4302-4309, Vol. 74, No. 9
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Nucleic Acid-Dependent Cross-Linking of the Nucleocapsid Protein of Sindbis Virus

Timothy L. Tellinghuisen and Richard J. Kuhn^*

Department of Biological Sciences, Purdue University, West Lafayette, Indiana 47907

Received 17 December 1999/Accepted 2 February 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The assembly of the alphavirus nucleocapsid core is a multistep event requiring the association of the nucleocapsid proteinwith nucleic acid and the subsequent oligomerization of capsidproteins into an assembled core particle. Although the mechanismof assembly has been investigated extensively both in vivo andin vitro, no intermediates in the core assembly pathway have beenidentified. Through the use of both truncated and mutant Sindbisvirus nucleocapsid proteins and a variety of cross-linking reagents,a possible nucleic acid-protein assembly intermediate has beendetected. The cross-linked species, a covalent dimer, has beendetected only in the presence of nucleic acid and with capsidproteins capable of binding nucleic acid. Optimum nucleic acid-dependentcross-linking was seen at a protein-to-nucleic-acid ratio identicalto that required for maximum binding of the capsid protein tonucleic acid. Identical results were observed when cross-linkingin vitro assembled core particles of both Sindbis and Ross Riverviruses. Purified cross-linked dimers of truncated proteins andof mutant proteins that failed to assemble were found to incorporateinto assembled core particles when present as minor componentsin assembly reactions, suggesting that the cross-linking trapsan authentic intermediate in nucleocapsid core assembly. EndoproteinaseLys-C mapping of the position of the cross-link indicated thatlysine 250 of one capsid protein was cross-linked to lysine 250of an adjacent capsid protein. Examination of the position ofthe cross-link in relation to the existing model of the nucleocapsidcore suggests that the cross-linked species is a cross-capsomerecontact between a pentamer and hexamer at the quasi-threefoldaxis or is a cross-capsomere contact between hexamers at the threefoldaxis of the icosahedral core particle and suggests several possibleassembly models involving a nucleic acid-bound dimer of capsidprotein as an early step in the assemblypathway.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The nucleocapsid core (NC) of Sindbis virus (SINV), the prototypical alphavirus, is a 410-Å-diameter T = 4 icosahedron composedof an 11,703-nucleotide genomic RNA surrounded by 240 copies ofa single nucleocapsid protein (CP) (22). Cryoelectron microscopyand image reconstruction analysis structures of several completealphavirus virions have been generated (1, 11, 19). Examinationof the NC within these particles demonstrates a series of pentamericand hexameric capsomeres that project ~40 Å off of the core surface.Based on the size and location of the capsomeres, the C-terminaldomain of the CP has been attributed to the density within theseprojections (1). The structure of the C-terminal protease domainof the CP of SINV has been solved to atomic resolution (5).Attempts at generating an atomic structure of the complete SINVand Ross River virus (RRV), or the NCs alone, have been unsuccessful(13; T. L. Tellinghuisen, R. J. Kuhn, and M. G. Rossmann, unpublishedresults). Structural information about the NC has been limitedto the combination of the cryoelectron microscopy image reconstructionsof complete virions and the numerous crystal structures of portionsof CP. Modeling of the atomic structure of the SINV CP into thecryoelectron density of the RRV suggests a possible orientationof the protein within the capsomeres (1). This model is supportedby recent work involving the fitting of the atomic structure ofthe C-terminal domain of the Semliki Forest virus CP into a 9-Åcryoelectron microscopy image reconstruction of the complete SFVvirion, which demonstrates a similar orientation of the CP inthe core (3; E. J. Mancini and S. D. Fuller, personal communication).The identification of a high-resolution structure of the NC ofSINV or RRV is of paramount importance in understanding the mechanismof coreassembly.

The mechanism of the alphavirus NC assembly, although extensively studied, is poorly understood. It is known from previousin vivo studies that immediately following translation and proteolysis,the CP is associated with the large subunit of the ribosome (12,20). It then associates with genomic RNA and rapidly assemblesinto NCs (21). The rapidity of NC formation has made the identificationof assembly intermediatesdifficult.

To circumvent the complexity of studying NC assembly in vivo, an in vitro assembly system for SINV core-like particles (CLPs)has been established using purified CP (24, 27). It was foundthat CLPs could be assembled in the in vitro system using a varietyof single-stranded DNA or RNA substrates. Furthermore, CLPs producedby these systems closely resembled cytoplasmic CLPs purified frominfected cells in size and shape when examined by negative-stainelectron microscopy. Despite intensive investigation using thesein vitro assembly systems, no intermediates in the NC assemblyprocess have been observed using CP (residues 19 to 264) (24).

During the characterization of the in vitro assembly system, several CP truncations that failed to assemble particles butwere competent for nucleic acid binding and incorporation intocore particles were identified (24). Truncated CPs that lackednucleic acid binding capability failed to incorporate into coreparticles. Additionally, no NC assembly was observed in the absenceof nucleic acid, as had previously been observed (27). Sincenucleic acid binding appears to be a requirement for NC assembly,analysis of the state of the CP bound to nucleic acid is veryimportant. Based on analytical ultracentrifugation and size exclusionchromatography, the SINV CP is monomeric in solution, despitenumerous crystallographic examples of dimeric forms of the protein(2, 4). Truncated or mutant proteins that fail to assemblecore particles but retain nucleic acid binding properties maytherefore identify intermediates in the assembly process. In thepresent study, the oligomerization of assembly-incompetent truncatedand mutant CPs in the presence of nucleic acid was examined bythe use of a variety of lysine-specific cross-linkingreagents.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

SINV and RRV CPs and nucleic acids. SINV and RRV CPs were expressed and purified as described previously (24). Truncations of the SINV CP were also expressedand purified as previously described (24). Proteins are identifiedby the abbreviation CP followed by the residues expressed in parentheses.Protein purity was typically 90 to 95% as estimated by silverstain sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) and analytical sizing column analysis. All proteinconcentrations reported are based on absorbance at 280 nm usingan extinction coefficient of 27,880 M¹ cm¹ for CP(19-264) and 22,190 M¹ cm¹ for CP(81-264). Concentrations based on extinction coefficientswere confirmed by a protein assay (Bio-Rad, Hercules, Calif.)to validate the calculated extinction coefficients for the proteins.The standard synthetic 48-mer DNA oligonucleotide used in assemblyassays was 5'-CCGTTAATGCATGTCGAGATATAAAGCATAAGGGACATGCATTAACGG-3'.Shorter oligonucleotides consisting of 18, 16, 14, 12, and 6 nucleotideswere 3' truncations of the standard assembly oligonucleotide.Transfer RNA substrates consisted of commercial preparations ofultrapure yeast tRNA (Boehringer Mannheim, Indianapolis, Ind.).Viral genomic RNA consisted of purified and uncapped in vitrotranscripts generated from the pToto64 SINV cDNA clone (18).

Nucleic acid binding. Binding of various CPs to DNA oligonucleotides or tRNA was conducted as described below. Equal molar amounts of nucleic acidand protein (approximately 2 nmol of each) were mixed at roomtemperature in buffer A (25 mM HEPES [pH 7.4], 100 mM potassiumacetate, 1.7 mM magnesium acetate) with a reaction volume of 25µl, unless otherwise noted. For concentration dependence experiments,DNA oligonucleotides were diluted in buffer A to the concentrationsshown in Fig. 2 and added as equal volumes (12.5 µl) to 400-µg/mlCP samples (12.5 µl) and were incubated for 10 min. Mock nucleicacid-bound samples contained 12.5 µl of 1-mg/ml CP and 12.5 µlof buffer A. The samples were then treated as describedbelow.

Cross-linking of CP. Chemical reagents used for cross-linking analysis were dimethyl suberimidate (DMS), dimethyl pimelimidate (DMP), and disuccinimidylsuberate (DSS) (Pierce, Rockford, Ill.). For cross-linking analyses,nucleic acid-bound or mock-bound CP(81-264) samples were cross-linkedwith DMS at room temperature. Initial titration of the amountof DMS required for maximal CP cross-linking was performed. Foroptimal cross-linking, DMS was added in two aliquots over thespan of 1 h to reach a final concentration of 0.75 mM. Reactionswere terminated by the addition of 200 mM glycine followed bya 15-min incubation. Conditions for crosslinking with DMP wereidentical to those used for DMS. Cross-linking with DSS was conductedsimilarly to that with DMS and DMP, except that DSS was addedin a single aliquot to a final concentration of 10 µM and thereaction mixtures were incubated for 30 min. Reactions with DSSwere terminated by a 15-min incubation in the presence of 200mM glycine. Where indicated, cross-linking reaction mixtures weretreated with 1 U of RNase-free DNase I (Ambion, Austin, Tex.)following cross-linking reagent neutralization. Cross-linkingconditions used with CP(19-264)L52D were identical to those describedfor CP(81-264). Cross-linking of CP was monitored by both SDS-PAGEon 12% polyacrylamide gels and size exclusion analysis using aSuperdex 75 (10/30; 22-ml bed volume) analytical column (AmershamPharmacia Biotech, Piscataway, N.J.) equilibrated with bufferA.

Removal of nucleic acid from cross-linking reaction mixtures. CP(81-264) at 1 mg/ml in 100 µl of buffer A was mixed at room temperature with 100 µl of a 1-mg/ml tRNA solution in bufferA. Samples were incubated for 10 min, and DMS was added in twoaliquots over the span of 1 h to reach a final concentration of0.75 mM. Following cross-linking, excess unreacted DMS was eliminatedby the incubation of the reaction mixtures in the presence ofglycine at a final concentration of 200 mM for 15 min. Sampleswere then treated with 2 µl of a 1-mg/ml stock of RNase A (Sigma,St. Louis, Mo.) at 37°C for 30 min. The reaction mixtures werethen brought to a final concentration of 1 M NaCl to remove residualnucleic acid from the proteins. Samples were then exchanged intobuffer A by buffer exchange in Centricon-10 centrifugal concentrators(Amicon, Beverly, Mass.).

In vitro capsid assembly. In vitro capsid assembly was performed as described previously (24). Briefly, equal molar amounts of CP and nucleic acidwere mixed in a final volume of 100 µl in buffer A at room temperature.Typical reaction mixtures contained 50 µl of 1-mg/ml CP (1.8 nmol)and 50 µl of 1-mg/ml 48-base assembly oligonucleotide (2 nmol)or 50 µl of 500-µg/ml tRNA (1.8 nmol). The reaction mixtures wereincubated for 30 min at room temperature, and the products wereassayed for the presence of CLPs as describedbelow.

Cross-linking of in vitro-assembled CLP. Following in vitro assembly of CLPs under the conditions described above, CLPs were purified by sucrose gradient sedimentationand concentrated by using Centricon-100 centrifugal concentratorsto a final concentration of 1 mg/ml in buffer A. For cross-linkingof purified CLPs, 50 µl of purified CLPs (approximately 1 mg/ml)was cross-linked and analyzed under conditions identical to thosedescribed for CPs bound to nucleicacid.

Incorporation of cross-linked dimers into CLP. Following removal of nucleic acid and exchange into buffer A, CP(19-264)L52D or CP(81-264) cross-linking reaction mixtureswere added (50 µl of 1 mg/ml stock) to wild-type CP(19-264) (50µl of 1 mg/ml) at room temperature to obtain a final protein concentrationof 1 mg/ml in a volume of 100 µl. Cross-linked protein stockscontained approximately 45% dimeric protein. The 48-mer assemblyoligonucleotide was then added at 1 mg/ml in a volume of 100 µl.The reaction mixtures were incubated at room temperature for 10min and then loaded onto 25% freeze-thaw sucrose gradients inbuffer A. Samples were centrifuged at 38,000 rpm for 90 min inan SW-41 rotor (Beckman, Palo Alto, Calif.) at 4°C. Gradientswere fractionated by hand into 1-ml aliquots, and samples wereexamined by Western blot analysis. For Western blot analysis,gradient fractions were separated by SDS-PAGE (12% polyacrylamide)and transferred to nitrocellulose membranes (Amersham). The membraneswere exposed to a polyclonal anticapsid rabbit antibody and thento a secondary anti-rabbit goat immunoglobulin G conjugated tohorseradish peroxidase (Sigma). Blots were subjected to chemoluminescentdetection using enhanced chemiluminescence reagents (Amersham)and exposed to X-rayfilm.

Cross-link mapping. The location of the cross-link was mapped using a variety of proteolytic techniques. CP(81-264), the minimum sequence of CPwith which nucleic acid-dependent cross-linking was observed,was used in initial cross-link mapping experiments. The locationof the cross-link observed in longer protein constructs and completeparticles was mapped as described for CP(81-264). For trypsinizationexperiments, CP(81-264) cross-linking reaction mixtures were incubatedfor 4 h at 37°C with 40 ng of tolylsulfonyl phenylalanyl chloromethylketone (TPCK)-treated trypsin (Sigma). Following digestion, proteolyticfragments were examined by SDS-PAGE (15% polyacrylamide gels)and staining with Coomassie brilliant blue R-250. For endoproteinaseLys-C mapping experiments, CP(81-264) cross-linking reaction productswere denatured and digested for 16 h at 37°C with 5 ng of sequencing-gradeendoproteinase Lys-C (Boehringer Mannheim). Following digestion,proteolytic fragments were examined by electrophoresis on Tricine-SDS-PAGEgels (20% polyacrylamide) and stained with Coomassie brilliantblue R-250. Proteolytic fragments were transferred to Immobilon-Ppolyvinylidene difluoride membranes (Millipore, Bedford, Mass.),and selected fragments were identified by amino-terminal proteinsequencing. In all mapping experiments, non-cross-linked samplesof CP served as a negativecontrol.

Mutagenesis of lysine 250. In vitro mutagenesis of lysine 250 to arginine (K250R) was performed by using the Quick Change mutagenesis system (Stratagene,La Jolla, Calif.). The manufacturer's standard procedure and conditionsas described in the system literature were used. Mutagenesis wasperformed in a pGEM capsid gene carrier plasmid (pGEMCap; generouslyprovided by Rushika Perera) and was followed by subcloning, usingPfu polymerase-based DNA amplification, into a suitable expressionvector. All clones and mutants were confirmed by double-strandedDNA dideoxy sequencing using Sequenase PCR-based sequencing (Amersham).The mutant K250R protein was purified as described above for CP(19-264).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

DMS cross-linking of CP(81-264) is nucleic acid dependent. Preliminary research into the development of the Escherichia coli-expressed protein in vitro assembly system for SINV andRRV core particles suggested that nucleic acid binding was a requiredstep in the assembly of the NC (24). Definition of the stateof the CP bound to nucleic acid was of paramount importance inunderstanding the early stages of the capsid assembly mechanism.To examine the state of the CP bound to nucleic acid, the minimumnucleic acid binding form of the CP, CP(81-264), was incubatedwith various nucleic acid substrates and the binding-reactionproducts were analyzed using a variety oftechniques.

Initial cross-linking experiments, designed to identify the state of CP(81-264) bound to nucleic acid, were performed withglutaraldehyde. Glutaraldehyde cross-linking of these binding-reactionproducts failed to generate a specific nucleic acid-dependentcross-linked species. Therefore, the use of more specific cross-linkingreagents was investigated. Specific chemical cross-linkers arelargely limited to lysine- and cysteine-specific reagents. Examinationof the sequence of the SINV CP, which lacks any cysteines, suggestedthe use of lysine-specific cross-linking reagents. A variety oflysine-specific imidoesters were assayed for the ability to inducenucleic acid-dependent cross-linking of CP(81-264). Imidoesterreagents of ~11 Å were capable of generating covalent dimers ofCP(81-264) in the presence of nucleicacid.

A nucleic acid-dependent cross-linking of CP(81-264) with DMS is shown in Fig. 1. In lane 2, CP(81-264) cross-linked withDMS in the absence of nucleic acid is seen as only a monomer.Cross-linking of CP(81-264) bound to the 48-mer assembly oligonucleotidewith DMS demonstrated two species, a dimeric cross-linked formof the CP and non-cross-linked monomeric CP (lane 4). Westernblot analysis of reaction products identical to those shown inFig. 1 indicated that both the observed monomeric and dimericCP forms were immunoreactive to anti-SINV CP antisera (data notshown). The maximum observed cross-linking of CP into dimer withDMS was approximately 45 to 50% of total input protein, basedon visual estimation of SDS-PAGE gels. Addition of DMS in excessof the optimum established conditions failed to generate significantlygreater amounts of dimeric protein but did induce the formationof higher-order nonspecific cross-linked species (data not shown).Additionally, truncations of the CP, incapable of binding nucleicacid, were not cross-linked into dimers using DMS in the presenceor absence of nucleic acid (data not shown). The cross-linkingefficiency was found to be equivalent across a wide range of proteinconcentrations from 2.5 µg/ml to 3.5 mg/ml.

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FIG. 1. Nucleic acid-dependent cross-linking of CP(81-264). Lanes: 1, electrophoretic mobility of CP(81-264) by SDS-PAGE (12% polyacrylamide) with Coomassie brilliant blue R-250 staining, with only monomeric CP evident (M); 2, CP(81-264) treated with DMS in the absence of nucleic acid; 3, CP(81-264) bound to an equal molar concentration of the 48-mer assembly oligonucleotide; 4, CP(81-264) bound to DNA, as in lane 3, but cross-linked with DMS [the presence of a dimeric form of CP(81-264) is evident (D)]; 5, sample identical to that in lane 3 but treated with RNase-free DNase I; 6, sample identical to that in lane 4 but treated with RNase-free DNase I. In lane 6, the dimeric form of CP(81-264) remains following nuclease treatment (D).

To demonstrate that the cross-link was between two protein molecules and not between CP and the DNA, products were treatedwith DNase I. Lanes 5 and 6 of Fig. 1 show the DNase I treatmentof samples identical to those in lanes 3 and 4. DNase I treatmentof cross-linked protein samples was unable to eliminate the observeddimeric form of the CP. Additional data suggested that the observedcross-link was not a CP-nucleic acid adduct, since only cross-linkedspecies consistent with the size of a dimer of CP(81-264) couldbe generated with a range of nucleic acid sizes (see Fig. 2B).

To further demonstrate the specificity and relevance of the observed nucleic acid-dependent cross-linking, the nucleic acidrequirements for cross-linking were examined in light of the previouslyobserved requirements for in vitro NC assembly (24). Varyingthe amount of nucleic acid used in the CP(81-264) binding reactionsprior to cross-linking with DMS demonstrated that the optimumcross-linking was observed with the same ratio of nucleic acidto protein required for optimum binding of CP(81-264) (Fig. 2A).More importantly, it was also the same as the optimum ratio ofCP(19-264) protein to nucleic acid required for CLP assembly (Fig.2A, lane 3). Cross-linking at 500 µg of oligonucleotide per ml(approximately 2 oligonucleotides per CP) was observed, but atsuboptimum levels (lane 2). Cross-linking at 240 and 120 µg ofoligonucleotide per ml (corresponding to approximately 1 and 0.5oligonucleotide per CP, respectively) demonstrated the maximumobserved cross-linking. This correlated well with previous estimatesthat a molar ratio of 1 to 2 CPs per 48-mer oligonucleotide wasoptimum for assembly of CLPs in vitro (24). Further dilutionof the oligonucleotide (corresponding to 4 proteins per oligonucleotideand higher ratios) showed decreased cross-linking.

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FIG. 2. Nucleic acid concentration and length requirements for DMS cross-linking of CP(81-264). (A) Lane 1 demonstrates the electrophoretic mobility of CP(81-264) on SDS-PAGE (12% polyacrylamide) with Coomassie R-250 staining, with only monomeric protein evident (M). Lanes 2 to 6 represent decreasing amounts of the 48-mer assembly oligonucleotide mixed with a fixed amount of CP(81-264) in the presence of DMS. The electrophoretic mobilities of the monomeric (M) and dimeric (D) forms of CP(81-264) are indicated. Note that the optimum cross-linking efficiency is seen in lane 3. (B) Lane 1 is identical to lane 1 in panel A, showing the migration of CP(81-264) alone. Lanes 2 through 7 represent cross-linking of CP(81-264) with DMS in the presence of equal molar concentrations of 3' truncations of the standard assembly oligonucleotide. Efficient cross-linking is observed in lanes 2 through 5. Only trace levels of dimeric CP are seen with the 12-mer oligonucleotide (lane 6), and no cross-linking is observed with the 6-mer oligonucleotide (lane 7). nt, nucleotides.

Study of the SINV in vitro assembly system indicated that a minimum length of oligonucleotide was necessary for CLP formation(24). To examine if this limitation for nucleic acid substratesexisted for cross-linking of CP(81-264), a series of truncationsof the 48-mer assembly oligonucleotide were assayed for theirability to induce the CP dimer. In Fig. 2B, analysis of thesetruncated assembly oligonucleotides in cross-linking reactionsis presented. The standard assembly oligonucleotide (Fig. 2B,lane 2) served as a positive control for cross-linking. Truncationsof the assembly oligonucleotide shorter than 14 nucleotides significantlyreduced or eliminated the observed cross-linking of CP(81-264)(lanes 6 and 7). Therefore, a minimum length requirement for cross-linkingwas observed, and this paralleled the requirement seen for invitro core assembly. tRNA and viral RNA, which are competent substratesfor in vitro core assembly, were capable of binding CP(81-264),and identical cross-linking of the protein with DMS was observed(data not shown). In all circumstances, the requirements of nucleicacid for cross-linking were similar to previous results for invitro CLP assembly (24).

Cross-linking is distance specific. DMS has an 11.0-Å cross-linking distance and specificity for lysine residues. To demonstrate that the observed nucleic acid-dependentcross-linking was not an artifact of the reagent used, an 11.4-Ålysine-specific reagent (DSS) having a different cross-linkingchemistry was selected. Figure 3, lanes 1 and 2, show the DMSnucleic acid-dependent cross-linking of CP(81-264). In lanes 3and 4, the nucleic acid-dependent cross-linking of CP(81-264)with DSS is shown. Cross-linking with DSS was identical to thatobserved with DMS, although an increased cross-linking efficiencywas observed. DSS was found to induce additional higher-ordercross-linked species (trimers and tetramers); however, these specieswere not dilution independent and probably involved nonspecificcrosslinking (data not shown). An additional cross-linking reagentwith identical chemical mechanism and lysine specificity to DMSbut with a shorter cross-linking distance (9.2 Å) was selectedto examine if the reagent cross-link distance observed with DMSwas critical for the observed cross-linking. DMP was found tobe incapable of cross-linking CP(81-264) in the absence or presenceof nucleic acid (Fig. 3, lanes 5 and 6) or under any conditionstested (data not shown). These observations suggested that reagentchemistry was not important for the observed cross-linking butthat the cross-linking distance of the reagent was critical. Itcould be concluded that the observed cross-link occurred betweentwo lysine residues approximately 11 Å apart on adjacent CPs associatedwith nucleic acid.

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FIG. 3. Reagent specificity and distance constraints of nucleic acid-dependent cross-linking of CP(81-264). Lanes 1, 3, and 5 demonstrate the electrophoretic mobility of CP(81-264 NCP) on SDS-PAGE (12% polyacrylamide) with Coomassie R-250 staining, with only monomeric protein evident (M). Lane 2 shows DMS (11 Å) cross-linking of CP(81-264) bound to the 48-mer assembly oligonucleotide, with dimeric CP(81-264) indicated (D). Lane 4 contains CP(81-264) cross-linked with DSS (11 Å) in the presence of the standard assembly oligonucleotide. Lane 6 shows the lack of cross-linking of CP(81-264) with DMP (9 Å) in the presence of the 48-mer oligonucleotide.

DMS cross-linking is observed in abortive core assembly reactions and assembled CLPs. The cross-linking results observed with the truncated CP(81-264) were extended to consideration of assembly-defective CP(19-264)CP mutants. Extensive mutagenesis of the SINV CP and analysisof these mutant viruses has suggested several regions of the proteinthat appear to be involved in the NC assembly process (9, 10,15, 16, 18, 25, 29). Several of these mutations clusternear the amino-terminal end of the CP in a region that has beenproposed to form an $alpha$ -helix (residues 38 to 55) based on modelingof the primary sequence into helical wheel plots (R. Perera, K.E. Owen, A. E. Gorbalenya, and R. J. Kuhn, unpublished data).The most striking feature of this putative helix is the presenceof two conserved leucine residues at positions 45 and 52 (SINVamino acid numbering), which are arranged on the same face ofthe helix. These residues may form a leucine zipper interactionmotif between two CPs. Mutation of leucine 52 to aspartic acid[CP(19-264)L52D] eliminated cytoplasmic NC formation in vivo.This mutant CP failed to assemble CLPs in the in vitro core assemblyassay. However, the protein retained nucleic acid binding, asdetermined by electrophoretic mobility shift assay (data not shown).Nucleic acid binding properties and cross-linking of CP(19-264)L52Dwere similar to that observed for the truncated CP(81-264) andare shown in Fig. 4, lanes 1 and 2. In addition, densitometrymeasurements of the products of multiple independent reactionsof both proteins suggested that cross-linking efficiencies wereidentical (data not shown).

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FIG. 4. Nucleic acid-dependent cross-linking of full-length CPs. Lanes: 1, assembly-defective mutant CP(19-264)L52D, demonstrating the electrophoretic mobility of this protein on SDS-PAGE (12% polyacrylamide) in the absence of cross-linking; 2, CP(19-264)L52D bound to the 48-mer DNA oligonucleotide and cross-linked with DMS (a dimeric form of the CP is visible [D]); 3, SDS-PAGE migration of monomeric CP(19-264) wild-type protein in assembled CLPs; 4, identical CLPs to those seen in lane 3, but the CLPs were cross-linked with DMS, and a dimeric form of the CP is visible; 5, SDS-PAGE migration of monomeric RRV CP(1-270) wild-type protein in assembled CLPs; 6, identical RRV CLPs to those seen in lane 5, but the CLPs were cross-linked with DMS, and a dimeric form of the RRV CP(1-270) is detectable.

Cross-linking of in vitro-assembled CLPs was examined to demonstrate whether the observed cross-linking of truncated and assembly-defectivemutant CPs represented a conformation of CPs seen in the assembledNC. In vitro-assembled CLPs were capable of being cross-linkedwith DMS (Fig. 4, lanes 3 and 4), whereas purified wild-type CP(19-264)in the absence of nucleic acid could not be cross-linked (datanot shown). Cross-linking of particles with DMP generated no dimericform of the CP (data not shown). Only dimeric forms of CP(19-264)were observed in particle cross-linking reactions, with no higher-ordercross-links detectable. Additionally, in vitro-assembled CLPsof RRV were capable of nucleic acid-dependent crosslinking (lanes5 and6).

Cross-linked dimers can incorporate into CLPs. Since truncated and mutant CPs had been previously shown to incorporate into CLPs when present in in vitro assembly reactionmixtures as minor components (24), it was of interest to determineif cross-linked dimers of these proteins had a similar activity.CP(81-264) and CP(19-264)L52D dimers were produced as describedabove. Cross-linked dimers were then added to standard in vitroassembly reaction mixtures as minor components [0.5 nmol of CP(81-264)dimer, representing approximately 20% of the total input protein],and the reaction products were analyzed for the incorporationof dimeric forms of the CP into CLPs. Figure 5 shows a Westernblot analysis of sucrose gradient sedimentation of core assembly/dimerincorporation reactions. In lanes 6 and 7 of Fig. 5A and lanes6 and 7 of Fig. 5B, dimeric CPs can be seen cosedimenting within vitro-assembled CLPs. It is interesting that the dimer formof CP(81-264) was preferentially incorporated into CLPs comparedwith the monomer form of the protein (Fig. 5A, compare lanes 1and 6); however, the reason for this specificity is unknown. Incontrol reactions where CLPs were first assembled and then incubatedwith identical amounts of cross-linked dimers to those used inthe incorporation assays, no cosedimentation of dimer and CLPwas observed (data not shown). This suggested that the dimer wasincorporated in the core and was not aggregating or binding tothe surface. The CP(19-264)L52D-containing CLPs sedimented ata position consistent with CP(19-264) in vitro-assembled CLPs,whereas particles containing CP(81-264) sedimented in a slightlyaltered position based on examination of the location of NC bandingin sucrose gradients (data not shown). Examination of these assemblyreaction mixtures and gradient-purified CLPs by electron microscopysuggested that the particles were identical in size and morphologyto control CLPs (data not shown). No defects or aberrations inthe structure of the dimer-incorporated CLPs were apparent atthe level of negative-stain electron microscopy. The incorporationof the dimer into core assembly reaction mixtures strongly suggeststhat the cross-linked dimer is a trapped intermediate in the assemblyprocess.

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FIG. 5. Capsid assembly in the presence of dimeric protein. (A) In vitro core assembly with SINV CP(19-264) and the 48-mer assembly oligonucleotide in the presence of cross-linked CP(81-264) assayed by sucrose density gradient sedimentation followed by fractionation and Western blot analysis. Numbers across the top of this panel correspond to gradient fractions presented top (fraction 1) to bottom (fraction 12). A peak corresponding to the position of gradient sedimentation of the in vitro-assembled CLPs can be clearly seen in fractions 6 through 8. Monomeric CP(81-264) is present only in the top three fractions of the gradient. Dimeric CP(81-264) can be seen in the top three fraction of the gradient, as well as comigrating with the assembled CLPs in fractions 6 through 8. (B) In vitro core assembly with SINV CP(19-264) and the 48-mer assembly oligonucleotide in the presence of cross-linked CP(19-264)L52D assayed by sucrose density gradient sedimentation followed by fractionation and Western blot analysis. All numbering of fractions is identical to that in panel A. CLPs sediment in a peak in fractions 6 through 8. CP(19-264)L52D dimer can be seen on the top of the gradient in fraction 1, as well as cosedimenting with CLPs in fractions 6 to 8. CLPs from the experiments in panels A and B were confirmed by negative-stain electron microscopy. In both cases, the CLPs had normal size and morphology.

Cross-link mapping. With the demonstration of functional relevance of the dimer based on the incorporation of cross-linked dimers into CLPs, thelocation of the cross-link was investigated. It had been shownpreviously that treatment of virus-isolated SINV CP with trypsincould produce a truncated CP containing residues 103 to 264 (23).Therefore, the CP(81-264) or CP(19-264) cross-linked dimer wastreated with trypsin. The product of this treatment retained thecross-link and had a mobility on SDS-PAGE consistent with thatof a dimer of approximately CP(103-264). This suggested that theobserved cross-link was localized to the carboxyl-terminal regionof CP from residues 103 to 264. Additional proteolysis experimentsusing endoproteinase Lys-C further localized the cross-link (Fig.6A). Endoproteinase Lys-C treatment of CP(81-264) generated asingle large fragment of approximately 9 kDa and numerous smallerfragments (Fig. 6B, lanes 3 and 4). Endoproteinase Lys-C digestionof CP(81-264) cross-linked dimers produced the digestion patternof CP(81-264) plus an additional fragment of approximately 18kDa. Amino-terminal sequencing of the 18-kDa band identified theposition of this fragment in the CP, suggested that the observedcross-link was located between two 9-kDa fragments, and implicatedlysine 250 as the side chain involved in the cross-link. Sincethe 9-kDa fragment contains only one lysine residue, the cross-linkerhad reacted with identical residues on two monomers. Similar proteolyticmapping of CP(19-264) cross-linked in assembled CLPs indicatedthe same lysine-250-to-lysine-250 cross-link. The presence ofthe cross-link in nucleic acid binding reaction mixtures and inassembled CLPs further indicated that the observed cross-linkingof CP(81-264) was identical to the cross-linking observed in particles,suggesting that the nucleic acid-bound form of the truncated proteinwas an authentic intermediate in assembly. To further confirmthe location of the cross-link, a substitution of lysine 250 toarginine was performed. Purified CP(19-264) and CP(81-264) carryingthe lysine-250-to-arginine mutation lost the ability to cross-linkin the presence of nucleic acid with DMS. Additional evidencefor the importance of lysine 250 to the observed cross-linkingcan be found in the cross-linking of the RRV CP in assembled CLPs(Fig. 4, lane 6), since lysine 250 is conserved between SINV andRRV.

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FIG. 6. Endoproteinase Lys-C mapping of the location of the CP cross-linking. (A) Schematic of SINV CP(81-264) used in the mapping experiments. Endoproteinase Lys-C cleavage sites in the CP are indicated by arrowheads. The single large, 9-kDa peptide fragment produced by Lys-C digestion, consisting of amino acids 150 to 264, is indicated by hatching. (B) A Tricine-SDS-PAGE gel (20% polyacrylamide) stained with Coomassie blue R-250, demonstrating the results of endoproteinase Lys-C digestion of CP(81-264) and cross-linked CP(81-264). Lanes: 1, electrophoretic mobility of CP(81-264); 2, cross-linked CP(81-264) in the presence of DNA; 3, sample identical to that in lane 1, except that the samples were digested with endoproteinase Lys-C (the 9-kDa fragment, shown schematically in panel A, is indicated [9 kDa]); 4, sample identical to that in lane 2 but digested with endoproteinase Lys-C (the 9-kDa digestion product seen in lane 3 is visible in this lane, as is the dimeric form of this fragment [18 kDa]).

Location of the CP dimer. A model identifying residues 114 to 264 of the CP in the NC found in mature virions has been previously suggested (1).This model of the core structure was generated by fitting theatomic structure of the SINV CP(114-264) into the cryoelectronmicroscopy image reconstruction electron density of the NC ofRRV (Fig. 7A to C). Examination of the orientation of CPs in thisfit is consistent with the side chains of Lys-250 having a separationof 11 Å (Fig. 7C). In this cryoelectron microscopy fit model,the side chain of Lys-250 is projected into the intercapsomerespace separating pentamers and hexamers (subunits A₁ and C₁ inFig. 7B) and, although not shown, between adjacent hexamers (subunitsB₁ and D₂ in Fig. 7B). It therefore seems likely that the dimeridentified using chemical cross-linking is similar in orientationto CPs found in the mature virion (Fig. 7D).

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FIG. 7. Dimer model of the alphavirus nucleocapsid core. (A) A surface-shaded representation of the alphavirus NC as determined by cryoelectron microscopy and image reconstruction and viewed down a twofold axis (1). The pentamer and hexamer capsomeres can be clearly seen, with one pentamer and one hexamer colored in lavender. (B) Depth-cued representation of the NC with a superimposed T = 4 lattice. One icosahedral unit lies within the triangle and includes four CP monomers (A₁, B₁, C₁, and D₁). Yellow numbers identify the icosahedral axes, and green symbols label the pseudoaxes. (C) The electron density (lavender) of the pentamer and hexamer shown in panel A fitted with the atomic structure of residues 114 to 264 of the SINV CP (C $alpha$ backbone shown in yellow). A single loop from each monomer extends beyond the electron density and contains lysine 250 at its most distal point. Two lysine 250 residues that are separated by approximately ~12 Å are joined by a red line that represents the chemical cross-link. (D) Schematic representation of the CP subunits shown in panel C. The cross-link shown in panel C links the two CPs denoted A₁ and C₁ into a dimer. The CPs denoted by B₁ and D₂ (not shown, but see panel B) represent a second dimer that would be found in the particle.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Investigation of alphavirus assembly has provided limited insight into the molecular details of the pathway, due at leastin part, to the complexity of the in vivo environment. Structuralapproaches using cryoelectron microscopy and X-ray crystallographyhave provided substantial information concerning the organizationof the mature virion, its internal NC, and the C-terminal domainof the CP. However, this represents a static picture of the virusand its components and has limited value in explaining the dynamicprocess of particle assembly. The complexity of examining capsidassembly in vivo has been circumvented by the development of anin vitro assembly system that utilizes purified CP and nucleicacid. The presence of an in vitro assembly system allows the examinationof only the core assembly process separated from the other stepsin virus assembly and other aspects of the virus lifecycle.

During the development and characterization of the in vitro assembly system, the importance of nucleic acid binding in theearly events of capsid assembly was identified (24). Severaltruncated and mutant forms of the SINV CP were shown to bind nucleicacid but not to assemble into core particles. These proteins werefound to be competent to incorporate into core particles whenadded to wild-type assembly reaction mixtures, suggesting thatthe nucleic acid-bound form of these truncated proteins representedan early step in the assembly process. Therefore, identificationof the form of the CP bound to nucleic acid was important in understandingthe early steps in capsid assembly. For several virus assemblysystems, chemical cross-linking has been used to identify an intermediatein particle assembly (14, 17, 30). Early chemical cross-linkingexperiments with SINV CLPs purified from virus particles and CPextracted from purified CLPs demonstrated that numerous cross-linkingreagents could generate oligomers of the CP (6-8). Additionally,it was shown that purified CP and CLPs had different cross-linkingpatterns when compared. A preliminary arrangement of CPs in theNC was postulated based on their reactivity with cross-linkingreagents of various cross-linking distances (6).

Analysis using cross-linking reagents to detect the oligomeric state of truncated CP bound to nucleic acid in in vitro assemblyreactions led to some interesting observations. SINV CP(81-264),as well as CP(19-264)L52D, was found to be DMS-cross-linking competentonly in the presence of nucleic acid under all conditions tested.This observation is supported by numerous experiments suggestingthat the purified SINV CP is a monomeric protein in solution andthat interaction with nucleic acid leads to oligomerization ofthe CP (24, 27). Nucleic acid-dependent cross-linking wasfound to occur only with lysine-specific cross-linking reagentshaving a cross-linking distance of approximately 11 Å, with shorterspanning reagents failing to generate any cross-linked products.Nucleic acid requirements for cross-linking were similar to previouslypublished requirements for in vitro particle assembly, with bothconcentration and length limitations observed (24). These similaritiesbetween nucleic acid-dependent cross-linking and NC assembly suggestthat the cross-linking species observed represents an intermediatein the assembly process. Additional evidence can be found in theobservation that assembled CLPs contain the same cross-linkedspecies as were observed with either the truncated or mutant CP.Similarly, RRV CLPs can be cross-linked into an analogous dimer,presumably because of the conservation of the lysine residue atthat position of the CP. Further demonstration of the validityof the observed cross-linked dimer as an intermediate in the assemblypathway was provided by the incorporation of cross-linked dimersinto assembled CLPs. The similarities between the requirementsof cross-linking and particle assembly and the demonstration thatidentical dimers could be cross-linked in assembled CLPs or incorporatedinto particles after cross-linking strongly suggests that theobserved cross-linking represents a valid NC assemblyintermediate.

Examination of the location and distance of the observed cross-link in both CLPs and assembly-defective CPs in the presenceof nucleic acid together with the previous model of the core providessome interesting insights (1). The most surprising featureobserved when the fit of the crystal structure of the C-terminaldomain of the SINV CP into the electron density of the cryoelectronmicroscopy reconstruction of RRV was examined was the fact thatthe side chain of lysine 250 projects outward from the pentamericand hexameric capsomeres of the core (Fig. 7). Thus, the CP dimerisolated using the DMS cross-linker is a pair of CPs that spanthe intercapsomere space and must be in contact at the base ofthe core or utilize nucleic acid to bridge across the twoproteins.

The pentamer and hexamer capsomeres, which project ~40 Å from the surface of the NC, have been modeled to contain the C-terminaldomain of the CP (residues 114 to 264) (1). The remaining N-terminalresidues of the CP would form the base and interior of the NCtogether with the genome RNA. The first 80 amino acids of theN-terminal region have 13 arginines and 3 lysines and are thereforeexpected to line the interior of the NC in contact with the negativelycharged genome RNA. Indeed, Wengler has suggested that bindingof nucleic acid to this region results in a conformational change,allowing further assembly to occur (26). Within the N-terminal80 residues is a sequence of approximately 20 residues that canbe modeled as an $alpha$ -helix and plays a role in the assembly of theNC (Perera et al., unpublished). Deletions and point mutants inthis $alpha$ -helix seriously affect core assembly in vivo and blockassembly in vitro. It has also been shown through molecular geneticexperiments that much of the N terminus, excluding the putativehelix region, can be removed and particles can still be produced,demonstrating significant plasticity in this region of the protein(10).

Based on the previous structure and molecular genetic experiments, one possible assembly pathway for the NC was the preassemblyof capsomeres followed by the recruitment of RNA. The bindingof RNA to the highly basic N terminus permitted the close approachof the N-terminal $alpha$ -helices that then oligomerized to join thecapsomeres to form the core. However, despite extensive investigation,no free capsomeres have been identified in the in vitro reactionmixtures or with CP alone (24, 27, 28). The cross-linkingdata presented in this paper suggest that rather than capsomeres,the initial assembly intermediate is that of a dimer bound tonucleic acid that spans the intercapsomere space. Two chemicallyidentical dimers, A-C and B-D, would be sufficient to build theT = 4 icosahedral nucleocapsid (Fig. 7D), although the natureof CP oligomerization following dimer formation is unknown. Thismodel of assembly matches the observed experimental data, whichprevious models, based on capsomere pre-assembly and subsequentoligomerization, do not. It is also analogous to the assemblyof several plant viruses, most notably cowpea chlorotic mottlevirus (30). However, in cowpea chlorotic mottle virus, intercapsomeredimers can form in the absence of nucleicacid.

Through the use of cross-linking reagents and assembly-defective mutant and truncated CPs, a potential artificially trappedassembly intermediate has been identified. The biological activityof the cross-linked dimer of these assembly-defective CPs hasbeen demonstrated by the incorporation of these cross-linked speciesinto CLPs using the in vitro assembly system. The mapping of thecross-link to lysine 250 and the examination of the location ofthis residue in the model of the NC suggests that the model represents,at least in part, the structure of the in vitro-assembled core.Although the cross-link at lysine 250 permits one to model theorientation of the CP in the dimeric state, the site and natureof the dimer interface have yet to be resolved. Additionally,the site and role of nucleic acid binding in capsid dimerizationare unclear. The identification of cross-linked dimers of theSINV CP has led to new insights and to the generation of novelmodels for the assembly of the alphavirusNC.

	ACKNOWLEDGMENTS

We acknowledge Thomas J. Smith for valuable assistance in development of cross-linking conditions. Assistance in protein sequenceanalysis and protease mapping from Mary Bower is also acknowledged.The gift of pGEMcap plasmid from Rushika Perera is acknowledged.Additionally, critical discussions with Michael Rossmann, SergeiPletnev, Suchetana Mukhopadhyay, Rushika Perera, Chris Jones,Manoj Kumar, and Ranjit Warrier are gratefullyacknowledged.

This research was supported by Public Health Service grant GM56279 from the National Institutes of Health. Additional fundingfrom the Lucille Markey Foundation for structural studies at PurdueUniversity is acknowledged. T.L.T. was supported, in part, byNIH biophysics training grantGM98296.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biological Sciences, Purdue University, West Lafayette, IN 47907. Phone:(765) 494-1164. Fax: (765) 496-1189. E-mail: rjkuhn{at}bragg.bio.purdue.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Cheng, R. H., R. J. Kuhn, N. H. Olson, M. G. Rossmann, H.-K. Choi, T. J. Smith, and T. S. Baker. 1995. Nucleocapsid and glycoprotein organization in an enveloped virus. Cell 80:621-630[CrossRef][Medline].

2. Choi, H.-K., S. Lee, Y.-P. Zhang, B. R. McKinney, G. Wengler, M. G. Rossmann, and R. J. Kuhn. 1996. Structural analysis of Sindbis virus capsid mutants involving assembly and catalysis. J. Mol. Biol. 262:151-167[CrossRef][Medline].

3. Choi, H.-K., G. Lu, S. Lee, G. Wengler, and M. G. Rossmann. 1997. The structure of Semliki Forest virus core protein. Proteins Struct. Funct. Genet. 27:345-359[CrossRef][Medline].

4. Choi, H.-K., L. Tong, W. Minor, P. Dumas, U. Boege, M. G. Rossmann, and G. Wengler. 1991. Structure of Sindbis virus core protein reveals a chymotrypsin-like serine proteinase and the organization of the virion. Nature 354:37-43[CrossRef][Medline].

5. Choi, H. K., L. Tong, W. Minor, P. Dumas, U. Boege, M. G. Rossmann, and G. Wengler. 1991. Structure of Sindbis virus core protein reveals a chymotrypsin-like serine proteinase and the organization of the virion. Nature (London) 354:37-43.

6. Coombs, K., and D. T. Brown. 1987. Organization of the Sindbis virus nucleocapsid as revealed by bifunctional cross-linking agents. J. Mol. Biol. 195:359-371[CrossRef][Medline].

7. Coombs, K., and D. T. Brown. 1987. Topological organization of Sindbis virus capsid protein in isolated nucleocapsids. Virus Res. 7:131-149[CrossRef][Medline].

8. Coombs, K. M., and D. T. Brown. 1989. Form-determining functions in Sindbis virus nucleocapsids: nucleosomelike organization of the nucleocapsid. J. Virol. 63:883-891[Abstract/Free Full Text].

9. Forsell, K., G. Griffiths, and H. Garoff. 1996. Preformed cytoplasmic nucleocapsids are not necessary for alphavirus budding. EMBO J. 15:6495-6505[Medline].

10. Forsell, K., M. Suomalainen, and H. Garoff. 1995. Structure-function relation of the NH2-terminal domain of the Semliki Forest virus capsid protein. J. Virol. 69:1556-1563[Abstract].

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24. Tellinghuisen, T. L., A. E. Hamburger, B. R. Fisher, R. Ostendorp, and R. J. Kuhn. 1999. In vitro assembly of alphavirus cores by using nucleocapsid protein expressed in Escherichia coli. J. Virol. 73:5309-5319[Abstract/Free Full Text].

25. Weiss, B., U. Geigenmüller-Gnirke, and S. Schlesinger. 1994. Interactions between Sindbis virus RNAs and a 68 amino acid derivative of the viral capsid protein further defines the capsid binding site. Nucleic Acids Res. 22:780-786[Abstract/Free Full Text].

26. Wengler, G. 1987. The mode of assembly of alphavirus cores implies a mechanism for the disassembly of the cores in the early stages of infection. Arch. Virol. 94:1-14[CrossRef][Medline].

27. Wengler, G., U. Boege, G. Wengler, H. Bischoff, and K. Wahn. 1982. The core protein of the alphavirus Sindbis virus assembles into core-like nucleoproteins with the viral genome RNA and with other single-stranded nucleic acids in vitro. Virology 118:401-410[CrossRef][Medline].

28. Wengler, G., G. Wengler, U. Boege, and K. Wahn. 1984. Establishment and analysis of a system which allows assembly and disassembly of alphavirus core-like particles under physiological condition in vitro. Virology 132:401-412[CrossRef][Medline].

29. Wengler, G., D. Würkner, and G. Wengler. 1992. Identification of a sequence element in the alphavirus core protein which mediates interaction of cores with ribosomes and the disassembly of cores. Virology 191:880-888[CrossRef][Medline].

30. Zhao, X., J. M. Fox, N. H. Olson, T. S. Baker, and M. J. Young. 1995. In vitro assembly of cowpea chlorotic mottle virus from coat protein expressed in E. coli and in vitro-transcribed viral cDNA. Virology 207:486-494[CrossRef][Medline].

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Clin. Vaccine Immunol.	ALL ASM JOURNALS

1.	Cheng, R. H., R. J. Kuhn, N. H. Olson, M. G. Rossmann, H.-K. Choi, T. J. Smith, and T. S. Baker. 1995. Nucleocapsid and glycoprotein organization in an enveloped virus. Cell 80:621-630[CrossRef][Medline].
2.	Choi, H.-K., S. Lee, Y.-P. Zhang, B. R. McKinney, G. Wengler, M. G. Rossmann, and R. J. Kuhn. 1996. Structural analysis of Sindbis virus capsid mutants involving assembly and catalysis. J. Mol. Biol. 262:151-167[CrossRef][Medline].
3.	Choi, H.-K., G. Lu, S. Lee, G. Wengler, and M. G. Rossmann. 1997. The structure of Semliki Forest virus core protein. Proteins Struct. Funct. Genet. 27:345-359[CrossRef][Medline].
4.	Choi, H.-K., L. Tong, W. Minor, P. Dumas, U. Boege, M. G. Rossmann, and G. Wengler. 1991. Structure of Sindbis virus core protein reveals a chymotrypsin-like serine proteinase and the organization of the virion. Nature 354:37-43[CrossRef][Medline].
5.	Choi, H. K., L. Tong, W. Minor, P. Dumas, U. Boege, M. G. Rossmann, and G. Wengler. 1991. Structure of Sindbis virus core protein reveals a chymotrypsin-like serine proteinase and the organization of the virion. Nature (London) 354:37-43.
6.	Coombs, K., and D. T. Brown. 1987. Organization of the Sindbis virus nucleocapsid as revealed by bifunctional cross-linking agents. J. Mol. Biol. 195:359-371[CrossRef][Medline].
7.	Coombs, K., and D. T. Brown. 1987. Topological organization of Sindbis virus capsid protein in isolated nucleocapsids. Virus Res. 7:131-149[CrossRef][Medline].
8.	Coombs, K. M., and D. T. Brown. 1989. Form-determining functions in Sindbis virus nucleocapsids: nucleosomelike organization of the nucleocapsid. J. Virol. 63:883-891[Abstract/Free Full Text].
9.	Forsell, K., G. Griffiths, and H. Garoff. 1996. Preformed cytoplasmic nucleocapsids are not necessary for alphavirus budding. EMBO J. 15:6495-6505[Medline].
10.	Forsell, K., M. Suomalainen, and H. Garoff. 1995. Structure-function relation of the NH2-terminal domain of the Semliki Forest virus capsid protein. J. Virol. 69:1556-1563[Abstract].
11.	Fuller, S. D., J. A. Berriman, S. J. Butcher, and B. E. Gowen. 1995. Low pH induces swiveling of the glycoprotein heterodimers in the Semliki Forest virus spike complex. Cell 81:715-725[CrossRef][Medline].
12.	Glanville, N., and J. Ulmanen. 1976. Biological activity of in vitro synthesized protein: binding of Semliki Forest virus capsid protein to the large ribosomal subunit. Biochem. Biophys. Res. Commun. 71:393-399[CrossRef][Medline].
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