RNA Binding Properties of Bunyamwera Virus Nucleocapsid Protein and Selective Binding to an Element in the 5' Terminus of the Negative-Sense S Segment

doi:10.1128/JVI.74.21.9946-9952.2000

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Journal of Virology, November 2000, p. 9946-9952, Vol. 74, No. 21
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

RNA Binding Properties of Bunyamwera Virus Nucleocapsid Protein and Selective Binding to an Element in the 5' Terminus of the Negative-Sense S Segment

Jane C. Osborne and Richard M. Elliott^*

Division of Virology, Institute of Biomedical and Life Sciences, University of Glasgow, Glasgow G11 5JR, Scotland

Received 27 March 2000/Accepted 28 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The genome of Bunyamwera virus (BUN) (family Bunyaviridae, genus Bunyavirus) comprises three negative-sense RNA segments whichact as transcriptional templates for the viral polymerase onlywhen encapsidated by the nucleocapsid protein (N). Previous studieshave suggested that the encapsidation signal may reside withinthe 5' terminus of each segment. The BUN N protein was expressedas a 6-histidine-tagged fusion protein in Escherichia coli andpurified by metal chelate chromatography. An RNA probe containingthe 5'-terminal 32 and 3'-terminal 33 bases of the BUN S (small)genome segment was used to investigate binding by the N proteinin vitro using gel mobility shift and filter binding assays. Onacrylamide gels a number of discrete RNA-N complexes were resolved,and analysis of filter binding data indicated a degree of cooperativityin N protein binding. RNA-N complexes were resistant to digestionwith up to 1 µg of RNase A per ml. Competition assays with a varietyof viral and nonviral RNAs identified a region within the 5' terminusof the BUN S segment for which N had a high preference for binding.This site may constitute the signal for initiation of encapsidationbyN.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Bunyamwera virus (BUN) is the prototype of the genus Bunyavirus and the family Bunyaviridae and possesses a single-strandednegative-sense tripartite RNA genome. The three RNA segments,termed L (large), M (medium), and S (small), encode six proteins.The L segment codes for the L protein, the viral RNA-dependentRNA polymerase, which is responsible for both transcribing andreplicating the genome RNAs. The M segment encodes the two virionglycoproteins, G1 and G2, and a nonstructural protein, NSm, asa polyprotein which is probably cotranslationally cleaved by hostproteases. The S segment encodes the nucleocapsid (N) proteinand, in an overlapping reading frame, a second nonstructural proteincalled NSs (reviewed in reference 8).

In common with other negative-sense RNA viruses, the bunyavirus genome RNA segments are replicated via full-length cRNAs termedantigenomes. Both the negative-sense genome and positive-senseantigenome RNAs are encapsidated by the N protein and are associatedwith the viral polymerase in ribonucleoprotein complexes callednucleocapsids. It is only within the nucleocapsid that the RNAis transcriptionally active. Bunyavirus genome and antigenomeRNAs contain highly conserved, complementary terminal sequencesthat may form panhandle structures in vivo and are probably responsiblefor the circular appearance of isolated nucleocapsids (19, 20,22, 26, 28).

Full-length genome and antigenome segments are usually the only RNAs that are encapsidated in the infected cell. Viral mRNAs,which are not encapsidated, are truncated at the 3' end and containa nontemplated capped primer on the 5' terminus (2, 4, 9,14, 21). It is therefore likely that the terminal sequencesof the genome and antigenome RNAs are involved in the encapsidationprocess. This theory is supported by the observation that an antisensechloramphenicol acetyltransferase gene flanked by BUN terminalsequences was successfully encapsidated by N and transcribed byL in an in vivo system (7). Raju and Kolakofsky (25) reportedthat in infected cells a minority of encapsidated bunyavirus transcriptseither had the 3'-terminal truncation similar to mRNA but notthe 5' primer sequence or were full-length transcripts containinga capped primer on the 5' terminus (26). Taken together, thesedata suggest that the encapsidation signal is probably withinthe 5' terminal sequence of genome and antigenomeRNAs.

Investigations concerning the N proteins of viruses in the Hantavirus (11, 29) and Tospovirus (27) genera of the Bunyaviridaehave shown that binding of the N proteins to RNA in in vitro assaysis essentially sequence nonspecific. However, Severson et al.(29) reported hantavirus N protein to have a preference forfull-length hantavirus S segment RNA over RNA comprising onlyinternal sequences, and Gött et al. (11) reported hantavirusN to have a preference for double-strandedRNA.

The BUN N protein is a 26.7-kDa basic protein of 233 amino acids that does not show any sequence similarity to the hantavirus(ca. 50-kDa) or tospovirus (ca. 29-kDa) N proteins. Like the analogousnucleocapsid proteins of all members of the Bunyaviridae family,it contains no RNA binding consensus sequence (8). In thispaper we describe investigations into the binding of bacteriallyexpressed BUN N protein to negative-sense BUN S segment RNA sequencesin vitro. We also provide an analysis of the relative selectivityof the binding of N to such sequences with the intent to constructa model for the selective encapsidation of full-length viral genomeand antigenomeRNA.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression and purification of BUN N protein. The BUN N open reading frame (ORF), from codon 2 to stop codon 234, was amplified by PCR using primers 5'GCCGCGGATCCATCGAGGGAAGGATTGAGTTGGAATTTand 5'GCCGCGTCGACTTACATGTTGATTCCGAA, which also contain, respectively,BamHI and SalI restriction enzyme sites (underlined). The DNAamplicon was digested with BamHI and SalI and cloned between theBamHI and SalI sites of pQE30 (Qiagen). Recombinant N was expressedas an N-terminally 6-histidine-tagged protein in Escherichia colistrain M15 by induction with 1 mM isopropyl- $beta$ -D-thiogalactopyranoside(IPTG). The bacteria were lysed by freeze-thawing and sonication,and N protein was purified under native conditions (23) by Ni-nitrilotriaceticacid (NTA) column chromatography (Bio-Rad Econosystem). Proteinimmobilized on the Ni-NTA column was washed with 50 mM sodiumphosphate buffer (pH 6.0) containing 300 mM NaCl and 10% glycerol,and N was eluted with a linear gradient of 0 to 500 mM imidazolein wash buffer. Fractions containing large amounts of N were elutedat around 250 mM imidazole, pooled, and dialyzed at 4°C against10 mM NaCl in 10 mM Tris-HCl (pH 8.0). The dialyzed protein wasconcentrated using a Vivaspin concentrator (molecular weight cutoff,10,000) (Vivascience) and stored at 4°C.

RNA transcription plasmids. pT7BUNS5'(32)/3'(33) contains cDNA to the precise 32 5'-terminal bases and 33 3'-terminal bases of the negative-sense S segment,linked by a 5-base sequence which creates a SmaI site, under controlof a T7 promoter in pUC119. BUNS5'(32)/3'(33) RNA was transcribedfollowing linearization with BbsI, and BUNS-5'(32) RNA was transcribedfollowing linearization with SmaI.

pTZBUNS3'(33/22) contains cDNA to the precise 33 3' terminal bases of the negative-sense BUN S segment under control of aT7 promoter and was constructed by inserting a 63-bp SmaI-XbaIfragment from pT7BUNS5'(32)/3'(33) into pTZ18. pT7BUNS3'(33/22)RNA was transcribed following linearization of the plasmid withBbsI.

pT7BUNSCAT contains a negative-sense chloramphenicol acetyltransferase gene flanked by the entire untranslated regions ofthe BUN S segment in pUC119 (7). BUNS5'(65) RNA was transcribedfollowing linearization of this plasmid with FauI, and BUNS5'(135)RNA was transcribed following linearization with Tsp509I.

The template for transcription of BUNS5'SL2 RNA was generated by annealing two oligonucleotides, 5'CTAATACGACTCACTATA (modifiedT7 promoter) and 5'CTAAATCAACATTATATTGTTAATGGTATTTTAATATAGTGAGTCGTATTAG,representing bases 23 to 56 of the BUN S 5'terminus.

ORF( $-$ ) RNA was generated from a PCR product produced by amplification of the N ORF from nucleotides 577 to 86 of the cDNAto which a T7 promoter was incorporated, using primers 5'CTAATACGACTCACTATAGATCCCGATTGCTAAGGGand 5'CTGCGAATTCATGATTGAGTTGGAATTTCACG. The product was linearizedwith MnlI and made blunt ended using T4 DNA polymerase beforebeing added to a transcription reaction mixture to generate an87-base RNA. ORF(+) RNA, also 87 bases in length, was generatedfrom a PCR product by amplification of the N ORF from nucleotides491 to 784 of the cDNA to which a T7 promoter was incorporated,using primers 5'CTAATACGACTCACTATAGATGGAGAGGAAG and 5'CTGCGGATCCTTACATGTTGATTCCGAATTTAGC.The DNA was linearized with BstYI before being added to a transcriptionreaction mixture. To generate double-stranded ORF (dsORF) RNA,ORF( $-$ ) and ORF(+) RNAs were heated together at 95°C for 5 minand 65°C for 10 min, and then annealed by cooling to 25°C over40 min. Figure 1 shows the regions of the BUN S segment representedby the in vitro-transcribed RNAs.

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FIG. 1. Location of RNA probes used in binding assays relative to the BUN S genome segment. All of the transcripts were initiated with a truncated T7 promoter and did not contain additional, nonviral nucleotides at their 5' ends, except for BUNS3'(33/22) which had 22 nucleotides of vector sequence (bent line).

In vitro transcription reactions. RNA transcripts were generated using the Megashortscript T7 in vitro transcription kit (Ambion). BUNS5'(32) RNA was made underthe standard reaction conditions recommended by the manufacturer.All other unlabeled transcripts were synthesized in 20-µl reactionvolumes containing 3.75 mM each nucleoside triphosphate, 5 µgof plasmid template DNA or 8 µg of oligonucleotide template DNA,1× transcription buffer, and 1 µl of enzyme mix (both Ambion)and incubated at 37°C for 4 to 6 h. ³²P-labeled riboprobes were synthesized in similar reaction mixturescontaining 3.75 mM each ATP, GTP, and UTP, 3.75 µM CTP, and 17pmol of [ $alpha$ -³²P]CTP (3,000 Ci/mmol). All reaction mixtures were then treatedwith 1 µl of DNase I (Ambion) for 15 min at 37°C, and unincorporatedNTPs removed with RNA Mini Quick spin columns (Roche MolecularDiagnostics). The transcripts were purified by acid phenol (pH4.5)-chloroform extraction and ethanol precipitation in the presenceof ammonium acetate on dryice.

RNA-protein binding reactions. ³²P-labeled riboprobes were heated at 90°C for 2 min and cooled on ice for 5 min before being incubated with purified N proteinin a 10-µl volume binding reaction based on that of Gött et al.(11) containing 1× binding buffer (10 mM HEPES [pH 7.3], 150mM NaCl, 20 mM KCl, 5 mM MgCl₂, 1 mM EDTA, 2 mM dithiothreitol[DTT], 10 U of rRNasin [Promega]) for 20 min at 30°C; N proteinwas the last component to be added. Control reaction mixtureslacking N contained an equivalent volume of 1× dialysis buffer.In competitive binding reactions the competitor RNA was mixedwith the riboprobe in the reaction prior to the addition of N.For gel mobility shift analysis, glycerol was added to the binding-reactionmixtures to 12.5% and the reaction products were separated byelectrophoresis on a 6% polyacrylamide gel plus 5% glycerol and0.5× Tris-borate-EDTA (TBE) at 200 V for 2 h at 4°C or on a 1%agarose gel plus 0.5× TBE at 200 V for 1 h at 4°C. After drying,the gels were analyzed by autoradiography or by using a PhosphorImager(Bio-Rad). For filter-binding assays, 90 µl of 1× binding bufferwas added and the reaction products were passed under vacuum througha BA85 nitrocellulose membrane filter (Schleicher & Schuell) thathad been presoaked with 1× binding buffer. The filter was washedwith 500 µl of 1× binding buffer under vacuum and dried, and radioactivitywas determined by Cerenkovcounting.

Western blotting. Purified N was subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) on a 15% polyacrylamide geland blotted onto a nitrocellulose membrane (Amersham Life Science)by using a semidry electrophoretic transfer apparatus. The membranewas blocked for 16 h with blocking buffer (phosphate-bufferedsaline [PBS] containing 10% nonfat milk and 0.1% Tween 20) andthen incubated in blocking buffer for 1 h with rabbit serum raisedagainst purified BUN (1:500 dilution). The membrane was washedfour times with PBS-0.1% Tween 20, incubated with protein A-horseradishperoxidase conjugate (1:1,000 dilution) in blocking buffer for1 h, washed four times as before, and incubated twice in 50 mMTris-HCl (pH 7.5) for 15 min each. Visualization was performedusing enhanced chemiluminescence (Amersham PharmaciaBiotech).

Northwestern blotting. Purified N was subjected to SDS-PAGE and blotting as described above. The membrane was washed twice with PBS and blocked withPBS plus 5% nonfat milk and 1 mM DTT for 16 h, four times with1× HBB (25 mM HEPES [pH 7.5], 25 mM NaCl, 5 mM MgCl₂, 10 mM DTT)for 15 min each, and once with hybridization buffer (RNA-proteinbinding buffer plus 0.5% Nonidet P-40) for 15 min. The membranewas then probed with 5 ml of hybridization buffer plus 5 × 10⁵ cpm of ³²P-labeled riboprobe and 40 U of rRNasin (Promega) at room temperaturefor 2 h, washed three times with hybridization buffer, and analyzedbyautoradiography.

RNase treatment. ³²P-labeled BUNS5'(32)/3'(33) riboprobe was incubated in the presence or absence of 800 ng of N protein in a standard bindingreaction. RNase A was added to the concentrations specified, andthe reaction mixtures were incubated at 37°C for 10 min. RNA wasextracted with acid phenol (pH 4.5)-chloroform and precipitatedwith ethanol in the presence of ammonium acetate on dry ice. TheRNA pellets were washed with 70% ethanol, resuspended in 5 µlof water, and boiled in 50% formamide, and the products were separatedby PAGE on a 6% polyacrylamide sequencing-type gel at 300 V. Afterbeing dried, the gel was analyzed byautoradiography.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Expression and purification of recombinant BUN N protein. The BUN N protein was expressed as an N-terminally 6-histidine-tagged protein in E. coli and purified under native conditionsby nickel affinity chromatography. The bulk of N was eluted byapproximately 250 mM imidazole. Eluted fractions were dialyzed,concentrated, and stored at 4°C, at which temperature N was typicallystable for approximately 3 weeks. Analysis of the preparationby SDS-PAGE with subsequent staining with Coomassie blue showeda single band at the expected size for His-tagged N protein (datanot shown). Further analysis by Western blotting using a rabbitpolyclonal antiserum raised against purified BUN virus confirmedthe identity of the protein as N (Fig. 2, lane 1). Analysis ofthe highly concentrated eluate from bacteria containing emptyparent plasmid and purified under similar conditions did not yieldany bands (lane 2). Western blot analysis of 10-fold-more N thanthat in lane 1 yielded two additional bands of higher molecularmass (lane 3). The intensity of these bands was unaffected followingtreatment of the protein with 5 mg of RNase A per ml prior toelectrophoresis (lane 4). This concentration of RNase A is morethan sufficient to digest RNA in bunyavirus nucleocapsids. Thus,we suggest that these bands represent homodimers and homotrimersof N and were not the result of two or three N molecules bindingto the same RNA molecule.

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FIG. 2. Characterization of expressed, histidine-tagged BUN N protein. A 220-ng (lanes 1 and 5) or 2.2-mg (lanes 3 and 4) sample of purified N protein was blotted onto a nitrocellulose membrane following SDS-PAGE; extracts of bacteria containing parent plasmid and subjected to the same purification protocol were run in lanes 2 and 6. The protein preparation in lane 4 was incubated with 5 mg of RNase A per ml before being loaded on the gel. Filters of lanes 1 to 4 were reacted with a polyclonal rabbit antiserum prepared against purified BUN and detected monomeric N (lane 1) and presumed oligomeric forms of N (lanes 3 and 4). No reaction with control lysate was observed (lane 2), and prior treatment with RNase A had no effect (lane 4). The filter of lanes 5 and 6 was reacted with ³²P-labeled BUNS5'(32)/3'(33) RNA, and the N band was revealed following autoradiography (lane 5); no bands were detected on the blot of the extract from control bacteria (lane 6).

RNA binding by N protein. The terminal sequences of each of the three bunyavirus genome segments have been implicated in encapsidation and are proposedto contain the site for nucleocapsid assembly (25). A 69-baseriboprobe designated BUNS5'(32)/3'(33) was generated to investigatewhether the recombinant N protein would bind the S-segment termini.This RNA corresponds to the exact terminal 32 bases of the 5'end and 33 bases of the 3' end of the genome-sense S segment (Fig.1). Samples (100 pg) of radiolabeled BUNS5'(32)/3'(33) riboprobewere incubated with increasing concentrations of N under reactionconditions based on those described by Gött et al. (11) andthen analyzed by polyacrylamide and agarose gel electrophoreticmobility shift assays (GEMSA), filter binding assays, and Northwesternblotting.

When GEMSA was performed using an acrylamide gel (Fig. 3), at low concentrations of N a small proportion of riboprobe wasshifted into a single band of higher molecular mass. At higherconcentrations of N the riboprobe was shifted into multiple highercomplexes, forming a ladder-like profile, which suggests sequentialfilling of binding sites on the RNA (3). The multiple bandsare interpreted as the result of riboprobe being bound by discretenumbers of N molecules. Further addition of protein resulted insaturation of the riboprobe, which was shifted toward the topof the gel. To investigate the saturated complexes further, identicalreactions were analyzed by agarose GEMSA (Fig. 4). In this assaythe saturated complexes ran into the gel and could be seen toreach a finite maximum size. To confirm that the mobility shiftsof the riboprobe were due to interaction with N, the protein wasshown to bind BUNS5'(32)/3'(33) RNA directly by Northwestern blotanalysis (Fig. 2, lane 5). No binding of the riboprobe was observedin a mock expression lane in which bacteria containing the emptyparent vector had been subjected to an identical induction andpurification regime (lane 6), suggesting that the shifts observedin the GEMSAs were not attributable to interaction with a nativebacterial protein. When N was replaced by bovine serum albumenin binding reactions, no shift of the riboprobe was observed,indicating that the mobility shift was specific for the N protein(Fig. 4).

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FIG. 3. Analysis of N-RNA binding by polyacrylamide GEMSA. A 100-pg sample of ³²P-labeled BUNS5'(32)/3'(33) RNA was incubated with different concentrations of N protein, as indicated, before being subjected to analysis on a polyacrylamide gel. In the presence of increasing concentrations of N, the riboprobe was shifted into multiple higher complexes in a ladder-like profile. At high concentrations of N, the riboprobe was shifted toward the top of the gel.

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FIG. 4. Analysis of N-RNA binding by agarose GEMSA. A 100-pg sample of ³²P-labeled BUNS5'(32)/3'(33) RNA was incubated with different concentrations of N protein, as indicated, before being subjected to analysis on an agarose gel. In the presence of N, the riboprobe was shifted into a higher band of finite maximum size. The two bands observed for the free riboprobe are thought to be due to secondary structure in the RNA. Replacement of N by bovine serum albumen (BSA) in the binding-reaction mixture did not result in a mobility shift of the probe.

Effect of ionic concentration on binding. Binding reaction mixtures were assembled in the presence of different concentrations of NaCl (0.15 to 2 M) and of MgCl₂ (0to 20 mM), and the products were analyzed by agarose GEMSA (Fig.5). Complex formation was not impaired by up to 0.5 M NaCl; athigher salt concentrations there was no evidence of dissociationof the complex, indicated by the lack of free riboprobe, but radioactivitywas smeared further up the gel. We assume that this is an electrophoresisartifact caused by the high salt concentration in the sample.Binding of N to the riboprobe was unaffected at the MgCl₂ concentrationsused (Fig. 5). These results suggest that electrostatic interactionsdo not play a major role in the binding event. The fact that theN-RNA complexes were stable at high salt concentrations also suggeststhat the binding is strong.

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FIG. 5. Effect of ionic strength on complex formation. Binding-reaction mixtures contained 100 pg of ³²P-labeled BUNS5'(32)/3'(33) RNA, 2,100 nM purified N protein, and different concentrations of NaCl or MgCl₂, as indicated, before being subjected to analysis by agarose GEMSA. Binding of N was evident, and no free riboprobe was observed for the range of NaCl and MgCl₂ concentrations tested. The increase in retardation coinciding with the increased NaCl concentrations is probably an effect of high salt concentrations on the movement of the complex through the gel.

Complexes are resistant to RNase. The RNA in bunyavirus nucleocapsids is relatively resistant to digestion by "reasonable concentrations" (12, 16) of RNaseA but is digested by 100 µg of RNase A per ml (19). To investigatewhether in vitro-assembled N-RNA complexes were resistant to RNaseA, BUNS5'(32)/3'(33) riboprobe was incubated in binding reactionseither with or without N and then different amounts of RNase Awere added and incubation was continued for 10 min at 37°C. Allreaction mixtures contained 20 U of RNasin RNase inhibitor (Promega),which is needed to inhibit any RNases present in the N proteinstock (and thus would otherwise digest the RNA before N was ableto bind); this amount of RNasin was considered to exert a nominaleffect on the amount of RNase A added (1 U of RNasin inhibits5 ng of RNase A by 50%; Promega). After phenol extraction theRNAs were analyzed by electrophoresis on a denaturing, sequencing-typepolyacrylamide gel. As shown in Fig. 6, RNA complexed with N wasresistant to 1 µg of RNase A per ml whereas the naked riboprobewas almost fully digested at this concentration. Neither complexednor naked riboprobe was resistant to 2.5 µg of RNase A per mlor higher concentrations.

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FIG. 6. Effect of RNase on N-RNA complexes. Binding reactions were performed in mixtures containing 100 pg of ³²P-labeled BUNS5'(32)/3'(33) RNA with or without 800 ng of N, and then different concentrations of RNase A were added and incubation was continued for 10 min at 37°C. Following phenol extraction and ethanol precipitation, the RNAs were resolved on a denaturing acrylamide gel. Complexes were resistant to 1 µg of RNase A per ml but not to 2.5 µg/ml, whereas most of the free riboprobe was digested by 1 µg of RNase A per ml.

Kinetics of N binding. The kinetics of binding of N to BUNS5'(32)/3'(33) RNA was measured by filter binding assays with a wider range of concentrationsof N than that used in GEMSA. Binding-reaction mixtures containing100 pg of radiolabeled riboprobe were passed through nitrocellulosemembranes under vacuum. Whereas free riboprobe passed throughthe membrane, riboprobe complexed with N was immobilized on it.The degree of binding could thus be measured as the proportionof radiolabeled RNA retained on the membrane by its associationwith N (Fig. 7a). Maximal binding was obtained with 180 ng ofN in the reaction, equivalent to a molar ratio of 1:1,500 (RNAto protein). The dissociation constant (K_d), which was calculatedas half-maximum binding, was approximately 7 × 10⁸ M. Analysis of binding kinetics using a Hill plot provides amathematical calculation of the degree of cooperativity in thebinding event (3). The gradient of the resulting line servesas a measure of the number of sites that are bound cooperatively.Analysis of the binding data in Fig. 7a by this technique gavethe results shown in Fig. 7c and yielded a gradient of approximately1.2, indicating that the binding event showed a degree of cooperativity(3).

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FIG. 7. Binding kinetics of purified N protein to RNA. (a and b) A 100-pg ³²P-labeled BUNS5'(32)/3'(33) (a) or BUNS5'(65) (b) RNA was incubated with increasing concentrations of N protein before being passed through a nitrocellulose filter. The retained labeled RNA was determined by scintillation counting and corrected by subtracting background counts of riboprobe in the absence of N. The two probes showed similar kinetics and yielded a K_d of approximately 7 × 10⁸ M, calculated as equal to 1/2 V_max. Error bars indicate the standard deviation from three replicates. (c) Hill plot of binding of N to BUNS5'(32)/3'(33) RNA (solid diamonds) and BUNS-5'(65) RNA (open squares). Linear regression was performed on the data points, yielding gradients of 1.2 for BUNS5'(32)/3'(33) RNA and 1.3 for BUNS-5'(65) RNA, indicating a low degree of cooperativity in both cases.

Competitive binding assays. The encapsidation signal for bunyavirus genome and antigenome segments is proposed to reside within the 5'-terminal sequences(12, 16, 25). We used a panel of RNAs in competitive filterbinding assays to investigate the presence of such a signal. Binding-reactionmixtures were assembled containing radiolabeled BUNS5'(32)/3'(33)riboprobe in the presence of a 1,000-fold mass excess of unlabeledcompetitor RNAs, which were mixed prior to the addition of N (Fig.8). These experiments would therefore provide a measure of thedegree of selectivity of N for the competitor RNA over BUNS5'(32)/3'(33)RNA. The results were expressed as the percentage of competitionshown by the competitor RNA for binding to N; a low value indicatesthat most of N is binding the riboprobe, and a high value indicatesthat there is competition for binding by the unlabeled RNA. Toensure that any competition observed was not due to loss of labeledriboprobe through RNase degradation, the competitor RNAs weretested for RNase contamination by incubation with the riboprobe,under binding conditions, followed by electrophoresis on a denaturingpolyacrylamide gel and autoradiography. No evidence of RNase degradationof the riboprobe was observed (data not shown).

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FIG. 8. Competitive binding assays using a panel of RNAs. A 100-pg sample of ³²P-labeled BUNS5'(32)/3'(33) RNA and 100 ng of unlabeled competitor RNA were mixed, prior to the addition of 350 nM purified N, in a standard binding reaction. After incubation, the mixture was passed through a nitrocellulose filter and the retained labeled RNA was determined by scintillation counting and corrected by subtracting background counts of riboprobe in the absence of N. Results are expressed as percent competition. Thus, 100% competition would indicate that N bound the competitor RNA exclusively and 0% competition would indicate that N bound the riboprobe exclusively. The competitor RNAs are described in Materials and Methods.

A 1,000-fold molar excess of the homologous RNA, BUNS5'(32)/3'(33), gave about 50% competition, whereas yeast RNA competedto less than 20% (Fig. 8). Higher levels of competition were observedwith competitor RNAs containing the 5' end of the BUN S segment.BUNS5'(32) and BUNS5'(135) RNAs, comprising the terminal 32 and135 bases, respectively, reduced retention of riboprobe by about75 to 80%. BUNS5'(65) RNA consists of the 5' terminal 65 basesof the BUN negative-sense S segment and is thus a similar lengthto BUNS5'(32)/3'(33). In the presence of a 1,000-fold excess ofthis competitor, the proportion of riboprobe retained droppedby approximately 97%, indicating a high degree of competition.However, an RNA comprising an internal region of the 5' end, BUNS5'SL2(bases 23 to 56), showed only 20%competition.

The binding kinetics of N to BUNS5'(65) RNA were measured by a filter binding assay (Fig. 7b) and shown to be similar to thoseof BUNS5'(32)/3'(33). Analysis of the binding data with BUNS5'(65)RNA yielded a similar Hill plot to that of BUNS5'(32)/3'(33) RNA(Fig. 7c).

BUNS3'(33/22) consists of the 33 terminal bases at the 3' end of the S segment and some vector sequences, and competed toa low level similar to that of yeast RNA. ORF( $-$ ) and ORF(+) RNAscomprise 87-base transcripts, genome and antigenome sense, respectively,representing a region of the N ORF which encodes a highly conserveddomain in the N protein. Neither of these RNAs competed more thanyeast RNA. dsORF RNA was generated by annealing the two single-strandedORF transcripts and was used to compare the preference of N fordsRNA and ssRNA. dsORF RNA competed only slightly more than thessRNAs and did not reach the high levels shown by competitorscontaining 5' terminalsequences.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have described experiments to study the RNA binding properties of BUN nucleocapsid protein in vitro. Recombinant BUN Nprotein was expressed as a His-tagged protein in bacteria andpurified by nickel affinity chromatography. N was reactive toantiserum raised against purified BUN and demonstrated bindingactivity for RNA containing the terminal sequences of the negative-senseS RNA segment, with a dissociation constant of 7 × 10⁸ M, similar to the value reported for hantavirus N protein (29).RNA binding reactions in the presence of increasing concentrationsof N, followed by polyacrylamide GEMSA, indicated the presenceof discrete complexes until the RNA was fully encapsidated. Althoughthe observed pattern might represent binding of RNA to misfoldedN protein, we think this unlikely since multiple bands of appropriatesizes are seen on Western blots (Fig. 2), suggesting that N iscapable of homo-oligomerizing. Analysis of the filter bindingassay data by a Hill plot (Fig. 7) indicated a low (nonsimultaneous)degree of cooperativity in the binding of N to the BUNS5'(32)/3'(33)RNA. Richmond et al. (27) reported RNA-binding by recombinanttomato spotted wilt virus N to be a cooperative event, as didGött et al. (11) for analysis of bacterially expressed hantavirusN protein binding, although neither group presented corroboratorydata, for example in the form of a Hillplot.

RNA-N protein complexes showed a finite maximum size when analyzed on an agarose gel (Fig. 4). We interpret this as indicatingthat N binds along the RNA as opposed to the RNA associating withpreformed multimers of N, whose size would be proportional tothe concentration of N in the reaction mixture. The RNA-N complexesformed in the binding reactions were shown to be resistant toa level of RNase A digestion similar to that of authentic nucleocapsids,indicating that they possess similarproperties.

We observed a discrepancy between the K_d calculated from filter binding data and the equivalent degree of binding in GEMSA:the concentration of N required for 50% maximum binding in thefilter binding assay was lower than that required in the gel shiftassay. Since this was a consistent observation, we assume thatit is because the N-RNA complexes were less stable during electrophoresis,particularly through a polyacrylamide gel. Filter binding wastherefore the preferred method for competitive binding assaysto investigate the selectivity of binding by N. Interpretationof the results was complicated by the finding that even in thepresence of a 1,000-fold excess of homologous unlabeled competitor,the retention of BUNS5'(32)/3'(33) riboprobe was decreased byonly 50%. The unexpected lower level of competition observed withthe homologous RNA may be due to interactions between the 5' and3' termini of BUNS5'(32)/3'(33) such that the labeled RNA is ableto base-pair with unlabeled homologous RNA to form multimers,thereby reducing the sensitivity of the assay. This phenomenonwould occur when the RNA possesses both termini on the samestrand.

We were able to identify the first 32 bases of the 5' negative-sense S segment as a region for which N possesses a preferenceover RNAs lacking this region. Analyses of the RNAs containing5'-terminal sequences by the Mfold program (18, 35) predictthe presence of a stem-loop structure, designated I, near the5' terminus (Fig. 9). It is possible that the observed preferencefor binding is provided by this putative stem-loop, which mightact as a signal for N to begin binding the segment RNA. BUNS5'(65)is predicted to form a second stem-loop, II (Fig. 9a), and stem-loopssimilar to stem-loop II are predicted in the first 65 bases ofthe 5' negative-sense termini of the other BUN segments (datanot shown). However, RNA comprising just stem-loop II (BUNS5'SL2RNA) competed similarly to yeast RNA and is therefore not thesole contributor of the high degree of competition seen with BUNS5'(65).In addition, Mfold does not predict that BUNS5'(135) containsstem-loop II, although stem loop I is still predicted (data notshown). BUNS3'(33/22), an RNA possessing the 3' terminus but lackingthe 5' terminus, did not demonstrate a greater degree of competitionthan yeast RNA, which suggests that the 3' terminus does not contributesignificantly to the selectivity observed for BUNS5'(32)/3'(33).The preference of N for the 5' terminus is unlikely to be dueto N binding dsRNA nonspecifically, since N did not possess ahigh preference for ORF dsRNA. Stem-loop I in the 5' terminusmight also have implications for the structure of the putativepanhandle involving the ends of the RNA segment, particularlyif this structure were retained after N binds, because loop Iresembles the hook structures that have been proposed in the 5'termini of influenza virus and Thogoto virus RNAs (10, 17,31).

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FIG. 9. Predicted secondary structure of the 5' terminus of BUN S segment RNA. Secondary structures of BUNS5'(65) (a) and BUNS5'(32) RNA (b) were predicted using Mfold (18, 35). The most energetically favorable structures are shown, and stem-loops I and II are indicated.

Normally only full-length genome and antigenome segments are encapsidated in bunyavirus-infected cells, and hence a mechanismmust exist to distinguish between these and viral mRNAs (or indeedcellular RNAs); it has been proposed that the presence of theadditional primer-derived bases at the 5' termini of viral mRNAsplays a role (25). We suggest that such additional bases mayaffect the secondary structure in the 5' terminus, and experimentsto test this hypothesis are under way. La Crosse bunyavirus Nprotein is reported to bind S segment-derived mRNA when N is presentat high concentrations in infected cells, providing a feedbackmechanism to regulate its own concentration (12), and this suggeststhat although authentic N is capable of binding RNAs other thangenomes and antigenomes, it can only do so when present at highconcentration. Competitive-binding experiments reported abovesuggest that BUN N is also capable of binding nonviral RNAs sinceyeast RNA could compete to a low but reproducible degree (Fig.8), which is presumably not sequencespecific.

Taken together, our observations may indicate two types of binding by N protein to RNA, selective or preferential bindingto the 5'-terminal region and nonspecific binding. Other proteinshave exhibited characteristics similar to those observed withBUN N. Heterogeneous nuclear ribonucleoproteins are capable ofboth preferential binding to certain sequences and less sequence-specificbinding at high concentrations, probably serving to hinder theformation of secondary structure in RNA (5, 6). Many positive-senseRNA virus core or coat proteins often possess the ability to selectivelybind specific sequences (13, 15, 32, 34), sometimes bindinghairpins in the 3' terminus, as well as binding RNA nonspecifically.Preferential binding to an encapsidation signal has also beenobserved for rabies virus (33) and human immunodeficiency virus(1).

The prediction of a binding site near the 5' terminus for which N is highly selective is in agreement with the suggestionof Kolakofsky and colleagues (12, 25), who envisaged a scenarioin which N binds a site in the 5' terminus of the segment RNAas it is being transcribed. Addition of the next N monomer couldoccur through its combined affinity for the RNA and the boundprotein, and in this regard, homotypic interactions between tomatospotted wilt virus N proteins have already been reported (30).Encapsidation of the RNA as it is being transcribed removes thenecessity for highly cooperative binding unless the transcriptionelongation event is progressing more quickly than the bindingof N to the nascentchain.

	ACKNOWLEDGMENTS

We thank Carol Noonan for assisting with protein purification, Ewan Dunn for supplying some of the transcription plasmids,and Paul Yeo for helpfuldiscussion.

J.C.O. was supported by a CASE studentship from BBSRC and Roche Products Ltd., and work in the laboratory of R.M.E. is supportedby grants from the Wellcome Trust and theMRC.

	FOOTNOTES

^* Corresponding author. Mailing address: Institute of Virology, University of Glasgow, Church St., Glasgow G11 5JR, Scotland.Phone: 44 141 330 4024. Fax: 44 141 337 2236. E-mail: r.elliott{at}vir.gla.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Allen, P., B. Collins, D. Brown, Z. Hostomsky, and L. Gold. 1996. A specific RNA structural motif mediates high affinity binding by the HIV-1 nucleocapsid protein (NCp7). Virology 225:306-315[CrossRef][Medline].

2. Bishop, D. H. L., M. E. Gay, and Y. Matsuoko. 1983. Non-viral heterogeneous sequences are present at the 5' ends of one species of snowshoe hare bunyavirus S complementary RNA. Nucleic Acids Res. 11:6409-6418[Abstract/Free Full Text].

3. Black, D. L., R. Chan, H. Min, J. Wang, and L. Bell. 1998. The electrophoretic mobility shift assay for RNA binding proteins, p. 109-136. In C. W. J. Smith (ed.), RNA:protein interactions Oxford University Press, Oxford, United Kingdom.

4. Bouloy, M., N. Pardigon, P. Vialet, S. Gerbaud, and M. Girad. 1990. Characterisation of the 5' and 3' ends of viral messenger RNAs isolated from BHK21 cells infected with Germiston virus (Bunyavirus). Virology 75:50-58.

5. Burd, C. G., and G. Dreyfuss. 1994. Conserved structures and diversity of functions of RNA-binding proteins. Science 265:615-621[Abstract/Free Full Text].

6. Burd, C. G., and G. Dreyfuss. 1994. RNA binding specificity of hnRNP A1: significance of hnRNP A1 high-affinity binding sites in pre-mRNA splicing. EMBO J. 13:1197-1204[Medline].

7. Dunn, E. F., D. C. Pritlove, H. Jin, and R. M. Elliott. 1995. Transcription of a recombinant Bunyavirus RNA template by transiently expressed Bunyavirus proteins. Virology 211:133-143[CrossRef][Medline].

8. Elliott, R. M. (ed.). 1996. The Bunyaviridae. Plenum Press, New York, N.Y.

9. Eshita, Y., B. Ericson, V. Romanowski, and D. H. L. Bishop. 1985. Analyses of the mRNA transcription processes of snowshoe hare bunyavirus S and M RNA species. J. Virol. 55:681-689[Abstract/Free Full Text].

10. Flick, R., G. Neumann, E. Hoffmann, E. Neumeier, and G. Hobom. 1996. Promoter elements in the influenza vRNA terminal structure. RNA 2:1046-1057[Abstract].

11. Gött, P., R. Stohwasser, P. Schnitzler, G. Darai, and E. K. F. Bautz. 1993. RNA binding of recombinant nucleocapsid proteins of hantaviruses. Virology 194:332-337[CrossRef][Medline].

12. Hacker, D., R. Raju, and D. Kolakofsky. 1989. La Crosse virus nucleocapsid protein controls its own synthesis in mosquito cells by encapsidating its mRNA. J. Virol. 63:5166-5174[Abstract/Free Full Text].

13. Hacker, D. L. 1995. Identification of a coat protein binding site on southern bean mosaic virus RNA. Virology 207:562-565[CrossRef][Medline].

14. Jin, H., and R. M. Elliott. 1993. Characterization of Bunyamwera virus S RNA that is transcribed and replicated by the L protein expressed from recombinant vaccinia virus. J. Virol. 67:1396-1404[Abstract/Free Full Text].

15. Khromykh, A. A., and E. G. Westaway. 1996. RNA binding properties of core protein of the flavivirus Kunjin. Arch. Virol. 141:685-699[CrossRef][Medline].

16. Kolakofsky, D., and D. Hacker. 1991. Bunyavirus RNA synthesis: genome transcription and replication. Curr. Top. Microbiol. Immunol. 169:143-159[Medline].

17. Leahy, M. B., J. T. Dessens, and P. A. Nuttall. 1997. Striking conformational similarities between the transcription promoters of Thogoto and influenza A viruses: evidence for intrastrand base pairing in the 5' promoter arm. J. Virol. 71:8352-8356[Abstract].

18. Mathews, D. H., J. Sabina, M. Zuker, and D. H. Turner. 1999. Expanded sequence dependence of thermodynamic parameters provides robust prediction of RNA secondary structure. J. Mol. Biol. 288:911-940[CrossRef][Medline].

19. Obijeski, J. F., D. H. L. Bishop, E. L. Palmer, and F. A. Murphy. 1976. Segmented genome and nucleocapsid of La Crosse virus. J. Virol. 20:664-675[Abstract/Free Full Text].

20. Pardigon, N., P. Vialat, M. Girard, and M. Bouloy. 1982. Panhandles and hairpin structures at the termini of Germiston virus (Bunyavirus). Virology 122:191-197[CrossRef][Medline].

21. Patterson, J. L., and D. Kolakofsky. 1984. Characterization of La Crosse virus small genome transcripts. J. Virol. 49:680-685[Abstract/Free Full Text].

22. Pettersson, R. F., and C. H. von Bonsdorf. 1975. Ribonucleoproteins of Uukuniemi virus are circular. J. Virol. 15:386-392[Abstract/Free Full Text].

23. Qiagen. 1997. The QIAexpressionist, 3rd ed. Qiagen, Hilden, Germany.

24. Raju, R., and D. Kolakofsky. 1986. Translational requirement of La Crosse virus S-mRNA synthesis: in vivo studies. J. Virol. 61:96-103.

25. Raju, R., and D. Kolakofsky. 1987. Unusual transcripts in La Crosse virus-infected cells and the site for nucleocapsid assembly. J. Virol. 61:667-672[Abstract/Free Full Text].

26. Raju, R., and D. Kolakofsky. 1989. The ends of La Crosse virus genome and antigenome RNAs within nucleocapsids are base paired. J. Virol. 63:122-128[Abstract/Free Full Text].

27. Richmond, K. E., K. Chenault, J. L. Sherwood, and T. L. German. 1998. Characterization of the nucleic acid binding properties of tomato spotted wilt virus nucleocapsid protein. Virology 248:6-11[CrossRef][Medline].

28. Samso, A., M. Bouloy, and C. Hannoun. 1975. Presence de ribonucleoproteins circulaires dans le virus Lumbo (Bunyavirus). C. R. Acad. Sci. Ser. D 280:779-782.

29. Severson, W., L. Partin, C. S. Schmaljohn, and C. B. Jonsson. 1999. Characterization of the Hantaan nucleocapsid protein-ribonucleic acid interaction. J. Biol. Chem. 274:33732-33739[Abstract/Free Full Text].

30. Uhrig, J. F., T.-R. Soellick, C. J. Minke, C. Philipp, J.-W. Kellmann, and P. H. Schreier. 1999. Homotypic interaction and multimerization of nucleocapsid protein of tomato spotted wilt tospovirus: identification and characterization of two interacting domains. Proc. Natl. Acad. Sci. USA 96:55-60[Abstract/Free Full Text].

31. Weber, F., O. Haller, and G. Kochs. 1997. Conserved vRNA end sequences of Thogoto-orthomyxovirus suggest a new panhandle structure. Arch. Virol. 142:1029-1033[CrossRef][Medline].

32. Wei, N., and T. J. Morris. 1991. Interactions between viral coat protein and a specific binding region on turnip crinkle virus RNA. J. Mol. Biol. 222:437-443[CrossRef][Medline].

33. Yang, J., D. C. Hooper, W. H. Wunner, H. Koprowski, B. Dietzschold, and Z. F. Fu. 1998. The specificity of rabies virus RNA encapsidation by nucleoprotein. Virology 242:107-117[CrossRef][Medline].

34. Zhou, M., A. K. Williams, S.-I. Chung, L. Wang, and E. W. Collisson. 1996. The infectious bronchitis virus nucleocapsid protein binds RNA sequences in the 3' terminus of the genome. Virology 217:191-199[CrossRef][Medline].

35. Zuker, M., D. H. Mathews, and D. H. Turner. 1999. Algorithms and thermodynamics for RNA secondary structure prediction: a practical guide. NATO ASI Ser. 70:11-43.

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1.	Allen, P., B. Collins, D. Brown, Z. Hostomsky, and L. Gold. 1996. A specific RNA structural motif mediates high affinity binding by the HIV-1 nucleocapsid protein (NCp7). Virology 225:306-315[CrossRef][Medline].
2.	Bishop, D. H. L., M. E. Gay, and Y. Matsuoko. 1983. Non-viral heterogeneous sequences are present at the 5' ends of one species of snowshoe hare bunyavirus S complementary RNA. Nucleic Acids Res. 11:6409-6418[Abstract/Free Full Text].
3.	Black, D. L., R. Chan, H. Min, J. Wang, and L. Bell. 1998. The electrophoretic mobility shift assay for RNA binding proteins, p. 109-136. In C. W. J. Smith (ed.), RNA:protein interactions Oxford University Press, Oxford, United Kingdom.
4.	Bouloy, M., N. Pardigon, P. Vialet, S. Gerbaud, and M. Girad. 1990. Characterisation of the 5' and 3' ends of viral messenger RNAs isolated from BHK21 cells infected with Germiston virus (Bunyavirus). Virology 75:50-58.
5.	Burd, C. G., and G. Dreyfuss. 1994. Conserved structures and diversity of functions of RNA-binding proteins. Science 265:615-621[Abstract/Free Full Text].
6.	Burd, C. G., and G. Dreyfuss. 1994. RNA binding specificity of hnRNP A1: significance of hnRNP A1 high-affinity binding sites in pre-mRNA splicing. EMBO J. 13:1197-1204[Medline].
7.	Dunn, E. F., D. C. Pritlove, H. Jin, and R. M. Elliott. 1995. Transcription of a recombinant Bunyavirus RNA template by transiently expressed Bunyavirus proteins. Virology 211:133-143[CrossRef][Medline].
8.	Elliott, R. M. (ed.). 1996. The Bunyaviridae. Plenum Press, New York, N.Y.
9.	Eshita, Y., B. Ericson, V. Romanowski, and D. H. L. Bishop. 1985. Analyses of the mRNA transcription processes of snowshoe hare bunyavirus S and M RNA species. J. Virol. 55:681-689[Abstract/Free Full Text].
10.	Flick, R., G. Neumann, E. Hoffmann, E. Neumeier, and G. Hobom. 1996. Promoter elements in the influenza vRNA terminal structure. RNA 2:1046-1057[Abstract].
11.	Gött, P., R. Stohwasser, P. Schnitzler, G. Darai, and E. K. F. Bautz. 1993. RNA binding of recombinant nucleocapsid proteins of hantaviruses. Virology 194:332-337[CrossRef][Medline].
12.	Hacker, D., R. Raju, and D. Kolakofsky. 1989. La Crosse virus nucleocapsid protein controls its own synthesis in mosquito cells by encapsidating its mRNA. J. Virol. 63:5166-5174[Abstract/Free Full Text].
13.	Hacker, D. L. 1995. Identification of a coat protein binding site on southern bean mosaic virus RNA. Virology 207:562-565[CrossRef][Medline].
14.	Jin, H., and R. M. Elliott. 1993. Characterization of Bunyamwera virus S RNA that is transcribed and replicated by the L protein expressed from recombinant vaccinia virus. J. Virol. 67:1396-1404[Abstract/Free Full Text].
15.	Khromykh, A. A., and E. G. Westaway. 1996. RNA binding properties of core protein of the flavivirus Kunjin. Arch. Virol. 141:685-699[CrossRef][Medline].
16.	Kolakofsky, D., and D. Hacker. 1991. Bunyavirus RNA synthesis: genome transcription and replication. Curr. Top. Microbiol. Immunol. 169:143-159[Medline].
17.	Leahy, M. B., J. T. Dessens, and P. A. Nuttall. 1997. Striking conformational similarities between the transcription promoters of Thogoto and influenza A viruses: evidence for intrastrand base pairing in the 5' promoter arm. J. Virol. 71:8352-8356[Abstract].
18.	Mathews, D. H., J. Sabina, M. Zuker, and D. H. Turner. 1999. Expanded sequence dependence of thermodynamic parameters provides robust prediction of RNA secondary structure. J. Mol. Biol. 288:911-940[CrossRef][Medline].
19.	Obijeski, J. F., D. H. L. Bishop, E. L. Palmer, and F. A. Murphy. 1976. Segmented genome and nucleocapsid of La Crosse virus. J. Virol. 20:664-675[Abstract/Free Full Text].
20.	Pardigon, N., P. Vialat, M. Girard, and M. Bouloy. 1982. Panhandles and hairpin structures at the termini of Germiston virus (Bunyavirus). Virology 122:191-197[CrossRef][Medline].
21.	Patterson, J. L., and D. Kolakofsky. 1984. Characterization of La Crosse virus small genome transcripts. J. Virol. 49:680-685[Abstract/Free Full Text].
22.	Pettersson, R. F., and C. H. von Bonsdorf. 1975. Ribonucleoproteins of Uukuniemi virus are circular. J. Virol. 15:386-392[Abstract/Free Full Text].
23.	Qiagen. 1997. The QIAexpressionist, 3rd ed. Qiagen, Hilden, Germany.
24.	Raju, R., and D. Kolakofsky. 1986. Translational requirement of La Crosse virus S-mRNA synthesis: in vivo studies. J. Virol. 61:96-103.
25.	Raju, R., and D. Kolakofsky. 1987. Unusual transcripts in La Crosse virus-infected cells and the site for nucleocapsid assembly. J. Virol. 61:667-672[Abstract/Free Full Text].
26.	Raju, R., and D. Kolakofsky. 1989. The ends of La Crosse virus genome and antigenome RNAs within nucleocapsids are base paired. J. Virol. 63:122-128[Abstract/Free Full Text].
27.	Richmond, K. E., K. Chenault, J. L. Sherwood, and T. L. German. 1998. Characterization of the nucleic acid binding properties of tomato spotted wilt virus nucleocapsid protein. Virology 248:6-11[CrossRef][Medline].
28.	Samso, A., M. Bouloy, and C. Hannoun. 1975. Presence de ribonucleoproteins circulaires dans le virus Lumbo (Bunyavirus). C. R. Acad. Sci. Ser. D 280:779-782.
29.	Severson, W., L. Partin, C. S. Schmaljohn, and C. B. Jonsson. 1999. Characterization of the Hantaan nucleocapsid protein-ribonucleic acid interaction. J. Biol. Chem. 274:33732-33739[Abstract/Free Full Text].
30.	Uhrig, J. F., T.-R. Soellick, C. J. Minke, C. Philipp, J.-W. Kellmann, and P. H. Schreier. 1999. Homotypic interaction and multimerization of nucleocapsid protein of tomato spotted wilt tospovirus: identification and characterization of two interacting domains. Proc. Natl. Acad. Sci. USA 96:55-60[Abstract/Free Full Text].
31.	Weber, F., O. Haller, and G. Kochs. 1997. Conserved vRNA end sequences of Thogoto-orthomyxovirus suggest a new panhandle structure. Arch. Virol. 142:1029-1033[CrossRef][Medline].
32.	Wei, N., and T. J. Morris. 1991. Interactions between viral coat protein and a specific binding region on turnip crinkle virus RNA. J. Mol. Biol. 222:437-443[CrossRef][Medline].
33.	Yang, J., D. C. Hooper, W. H. Wunner, H. Koprowski, B. Dietzschold, and Z. F. Fu. 1998. The specificity of rabies virus RNA encapsidation by nucleoprotein. Virology 242:107-117[CrossRef][Medline].
34.	Zhou, M., A. K. Williams, S.-I. Chung, L. Wang, and E. W. Collisson. 1996. The infectious bronchitis virus nucleocapsid protein binds RNA sequences in the 3' terminus of the genome. Virology 217:191-199[CrossRef][Medline].
35.	Zuker, M., D. H. Mathews, and D. H. Turner. 1999. Algorithms and thermodynamics for RNA secondary structure prediction: a practical guide. NATO ASI Ser. 70:11-43.