The Exceptionally Large Genome of Hendra Virus: Support for Creation of a New Genus within the Family Paramyxoviridae

doi:10.1128/JVI.74.21.9972-9979.2000

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Journal of Virology, November 2000, p. 9972-9979, Vol. 74, No. 21
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Exceptionally Large Genome of Hendra Virus: Support for Creation of a New Genus within the Family Paramyxoviridae

Lin-Fa Wang,^* Meng Yu, Eric Hansson, L. Ian Pritchard, Brian Shiell, Wojtek P. Michalski, and Bryan T. Eaton

CSIRO Livestock Industries, Australian Animal Health Laboratory, Geelong, Victoria 3220, Australia

Received 16 May 2000/Accepted 15 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

An outbreak of acute respiratory disease in Hendra, a suburb of Brisbane, Australia, in September 1994 resulted in the deathsof 14 racing horses and a horse trainer. The causative agent wasa new member of the family Paramyxoviridae. The virus was originallycalled Equine morbillivirus but was renamed Hendra virus (HeV)when molecular characterization highlighted differences betweenit and members of the genus Morbillivirus. Less than 5 years later,the closely related Nipah virus (NiV) emerged in Malaysia, spreadrapidly through the pig population, and caused the deaths of over100 people. We report the characterization of the HeV L gene andprotein, the genome termini, and gene boundary sequences, thuscompleting the HeV genome sequence. In the highly conserved regionof the L protein, the HeV sequence GDNE differs from the GDNQfound in almost all other nonsegmented negative-strand (NNS) RNAviruses. HeV has an absolutely conserved intergenic trinucleotidesequence, 3'-GAA-5', and highly conserved transcription initiationand termination sequences similar to those of respiroviruses andmorbilliviruses. The large genome size (18,234 nucleotides), theunique complementary genome terminal sequences of HeV, and thelimited homology with other members of the Paramyxoviridae suggestthat HeV, together with NiV, should be classified in a new genusin this family. The large genome of HeV also fills a gap in thespectrum of genome sizes observed with NNS RNA virus genomes.As such, it provides a further piece in the puzzle of NNS RNAvirusevolution.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Although they manifest diverse biological properties, viruses in the families Filoviridae, Paramyxoviridae, Rhabdoviridae,and Bornaviridae all contain a nonsegmented negative-strand (NNS)RNA genome and share features of genome organization. These facts,together with similarities in domain structure and sequence ofthe viral polymerase proteins, suggest a close phylogenetic relationship.The four families are now grouped taxonomically in the order Mononegavirales,the first taxon above family level to be recognized in virus taxonomy(23, 25). The genome size of viruses in the order varies significantly,ranging from 8.9 kb in the Bornaviridae to 19.1 kb in the Filoviridae.Members of the Rhabdoviridae and Paramyxoviridae have intermediategenome sizes, 10.8 to 14.9 kb and 15.1 to 15.9 kb, respectively.Two interesting observations can be made from the comparison ofgenome sizes. First, there is no overlap of genome size betweenvirus families. Second, genome size ranges differ significantlybetween the two families in which multiple genera have been defined,the Rhabdoviridae and Paramyxoviridae. Within the Rhabdoviridae,genome length can vary more than 40%, whereas variation withinthe Paramyxoviridae is no more than 5%. Thus, paramyxoviruses,especially those in the subfamily Paramyxovirinae, have traditionallybeen described as having a "uniform genome size" (23, 27).The universality of this feature is now challenged with the discovery,reported here, of a much larger genome for Hendra virus(HeV).

Members of the family Paramyxoviridae include highly contagious human and animal pathogens such as human parainfluenza viruses,Measles virus, Canine distemper virus, Rinderpest virus, Mumpsvirus, Newcastle disease virus (NDV), Human respiratory syncytialvirus, and Turkey rhinotracheitis virus. Classification withinthe family has undergone major changes in recent years, and thecurrent taxonomy (17, 24, 27) divides the family into twosubfamilies, Paramyxovirinae and Pneumovirinae. The Paramyxovirinaeinclude three genera, Respirovirus (formerly known as Paramyxovirus),Morbillivirus, and Rubulavirus, whereas the Pneumovirinae containstwo genera, Pneumovirus and Metapneumovirus.

HeV was the causative agent of an explosive outbreak of a respiratory disease that resulted in the deaths of 14 horses andone human in a 2-week period in September 1994 in Hendra, a suburbof Brisbane, Australia (19). The virus was also responsiblefor a fatal human case of encephalitis in 1995, the infectionalmost certainly being acquired during necropsy of two horsesthat had died as a result of HeV infection 13 months previously(20). In January 1999, an additional fatal equine case was reportedin North Queensland (13). Serological surveys and virus isolationstudies indicated that flying foxes (fruit bats) in the genusPteropus are likely to be the natural host of this new virus (11,16, 34).

In March 1999, a virus closely related to HeV emerged in Malaysia, spread rapidly via the respiratory route through the pigpopulation, and caused the death by encephalitis of over 100 people.Efforts to control the spread of the pathogen, Nipah virus (NiV),included the culling of over 1 million pigs (5, 6). NiVis closely related to HeV, and antibodies raised against one viruscan neutralize the other in serum neutralization tests, albeitwith reduced efficiency (5, 12). Positive antibody responsesto NiV have been recorded in the Malaysian fruit bat population(8).

In addition to these two viruses, several other newly emerged Mononegavirales members of bat origin have been identified.These include Australian bat lyssavirus (9) and Menangle virus(21). Australian bat lyssavirus is closely related to rabiesvirus and was responsible for the death of a bat handler in 1996(1). Menangle virus caused fetal death and abortion in pigsand respiratory disease in humans (4, 21). It appears tobe a member of the Rubulavirus genus (M. Westenberg, personalcommunication). A new member of the Paramyxoviridae has recentlybeen isolated from bat urine in Malaysia, and it displays someantigenic cross-reactivity with Menangle virus (K. Chua, personalcommunication).

Tidona et al. (30) reported the isolation and characterization of a novel virus, Tupaia paramyxovirus (TPMV), from treeshrews, and Renshaw et al. (26) recently published the molecularcharacterization of the Salem virus, yet another novel paramyxovirusisolated from horses. These two new viruses are phylogeneticallyrelated to each other and to HeV and morbilliviruses. The isolationof seven new viruses, at least four of which are zoonotic andfive of which appear to have originated from fruit bats, opensa new and exciting era in the investigation of the natural historyof Paramyxoviridae and NNS RNA viruses ingeneral.

In this paper, we report the molecular characterization of the HeV L gene, which encodes the RNA polymerase, and determinethe sequence of the genome termini and gene boundaries and thuscomplete the sequence of the largest genome in the Paramyxoviridaeto be described. Important molecular features will be summarizedto support the establishment of a new genus for HeV and NiV withinthe subfamily Paramyxovirinae.

	MATERIALS AND METHODS

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Genome sequencing. The construction and screening of a cDNA library from purified viral genomic RNA have been described previously (33). Briefly,HeV was purified by zonal centrifugation in sucrose gradients,and genomic RNA was isolated using standard methods. The TimeSavercDNA Synthesis Kit (Pharmacia) was used to make total cDNA byusing random priming followed by the addition of an EcoRI adaptorand cloning into the pZEr0-1 vector (Invitrogen). A genome walkingstrategy was used to isolate specific clones by colony hybridization.DNA sequencing was performed by a combination of manual sequencingwith the Sequenase Kit (USB) and automatic sequencing using theBig-Dye Dideoxyl Termination Cycle Sequencing kit (Pharmacia)and the ABI 377 Sequencer. Each nucleotide position was sequencedat least twice, either by sequencing overlapping clones or bysequencing the opposite strand of the same clone. Sequence confirmationby direct sequencing of PCR fragments without cloning was alsocarried out for several regions of importance. Sequences wereanalyzed and aligned using the software package, including CloneManager 5 and Align Plus 4, from S & E Software (Durham, N.C.)as described previously (33).

Cloning and sequencing of genome termini. Two different methods were used to determine genome end sequences. (i) For inverse PCR, purified viral genomic RNA was denaturedat 100°C for 40 s in the presence of deionized formamide and digestedwith tobacco acid pyrophosphatase (Epicentre Technologies) accordingto the manufacturer's instructions. The RNA was then phenol-chloroformextracted and ethanol precipitated at $-$ 70°C for 60 min. The 5'and 3' ends of the genomic RNA were ligated using RNase-free T4RNA Ligase (Promega) according to the manufacturer's instructions.Genomic RNA was again phenol-chloroform extracted and ethanolprecipitated. First-strand cDNA synthesis was performed with genome-specificprimers by using the SuperScript preamplification system (LifeTechnologies). PCR fragments incorporating the 5' and 3' endsof the viral genome were amplified and sequenced using genomespecific primers. (ii) For rapid amplification of cDNA ends, first-strandcDNA synthesis was performed using SuperScript II (Life Technologies)and virus-specific primer, followed by ligation of anchor (annealedfrom the top strand, 5'-CTAAT ACGAC TCACT ATAGG GCTCG AGCGC CCGCCCGGGC AGGT-3', and the 5'-phosphorylated bottom strand, 5'-ACCTGCCC-3') using T4 RNA ligase (New England Bio-Labs). SubsequentPCR amplifications were carried out using a combination of virus-specificprimers and two nested primers annealing to the anchor (AP1, 5'-GGATCCTAAT ACGAC TCACT ATAGG GC; AP2, 5'-AATAG GGCTC GAGCG GC). PCRproducts were then cloned as blunt-end fragments into the EcoRVsite of pZEr0-1 vector (Invitrogen) for sequence determination.A total of 24 independent clones weresequenced.

Production of monospecific antibodies in rabbits. A recombinant polypeptide corresponding to amino acid residues 245 to 517 of the deduced L protein was expressed in Escherichiacoli by using the pRSET vector as described previously (32).Approximately 1.5 mg of the recombinant protein was purified usingpreparative sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE), and the band of interest was visualized in ice-cold0.3 M KCl, cut out, and sliced into 2- by 2-mm pieces, followedby passive elution in 50 mM NH₄HCO₃ containing 0.1% SDS. Elutedprotein solution (0.5 ml at 0.5 mg/ml) was mixed with an equalvolume of Freund's incomplete adjuvant and used to immunize rabbits.The same injection was repeated 4 weeks later, followed by a thirdinjection 6 weeks later without adjuvant. Antibody titers andspecificity were determined by enzyme-linked immunosorbent assayand Western blotting using both recombinant antigens and purifiedvirusproteins.

Peptide mapping by in situ enzymatic digestion and mass spectrometry. An adaptation of the method described by Moritz et al. (18) was employed to obtain internal amino acid sequence and massspectrometry data. Approximately 200 µg of purified virus wasinactivated at 100°C for 5 min with 2% SDS and 3% dithiothreitol.Following electrophoresis, a stained band identified as the Lprotein (approximately 200 kDa) was excised from the gel and fragmentswere cut into 2-mm pieces and washed with 2 M NH₄HCO₃-50% acetonitrilefor 30 min. Gel pieces were dried and rehydrated in 50 mM Tris-HCl-1mM EDTA-6% acetonitrile (pH 8.5). Endoproteinase Lys-C (sequencinggrade; Wako) was added at an enzyme-to-substrate ratio of approximately1:10, and gels were incubated overnight at 37°C. After centrifugation,supernatant fluids containing peptides were removed. Gel pieceswere reextracted with 1% trifluoroacetic acid for 30 min withsonication, and after centrifugation, gel pieces were washed againwith 0.05% trifluoroacetic acid-80% acetonitrile for 30 min. Supernatantfluids were combined and concentrated, and peptides were separatedusing reverse-phase chromatography as previously described (33).Electrospray ionization mass spectrometry (ESI-MS) analysis ofLys-C digests was performed on a Finnigan LCQ instrument witha Hewlett-Packard 1090 HPLC. The Prospector MS-FIT program wasset to consider the following modifications: phosphorylation ofserine, threonine, and tyrosine; oxidation of methionine; N-terminalacetylation of unmodified cysteine; and 200.00 ppm masstolerance.

Nuecleotide sequence accession number. The sequence reported in this paper has been deposited in the GenBank database (accession no. AF017149).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Sequence analysis of the L gene and protein. A total of 21 overlapping cDNA clones covering the entire coding region of L gene were isolated from the cDNA library. Highlyconserved transcriptional start and stop signals were identified,and the size of L gene mRNA was predicted to be 6,955 nucleotides(nt). Sequence analysis revealed a single long open reading framecoding for a large protein of 2,244 amino acids (aa) with a calculatedmolecular mass of 257,280 Da. The identity of the L gene was confirmedusing two different approaches. Firstly, a monospecific antiserumraised to a portion of the L protein (aa 245 to 517) expressedin E. coli was used in Western blotting to identify the proteinin purified virus. The antiserum specifically reacted with a proteinwhose apparent molecular mass exceeded 200 kDa (data not shown).Secondly, peptides derived from the putative L protein band byLys-C digestion and separated by reverse-phase chromatographywere analyzed by mass spectrometry. A total of 47 masses was identified,and a majority (59%) matched those of the L protein sequence deducedfrom cDNA clones (Table 1).

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TABLE 1. Mass spectrometry analysis of Lys-C-digested peptides of HeV L protein

The first AUG codon in the HeV L gene was located at nt 24 in the same reading frame as that encoding the L protein. However,there were eight in-frame stop codons existing between this andthe second AUG codon at nt 154. The use of this second AUG codonas the initiation site of HeV L gene translation was supportedby the conserved N-terminal amino acid sequence of the deducedL protein in comparison with those of morbilliviruses and respiroviruses(data not shown). The 5' untranslated region (UTR) of the HeVL gene was therefore 153 nt in length (Table 2). On the otherhand, the 3' UTR of the HeV L gene (67 nt) was very similar insize to those of morbilliviruses (varying from 65 to 69 nt) andrespiroviruses (71 to 85 nt).

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TABLE 2. Comparison of L gene features of HeV and selected Paramyxovirinae members

The HeV L protein was rich in leucine and isoleucine (19.3%, which is more than 1.3 times that of an average protein) andcarried a net positive charge of +37 at neutral pH. The lineardomain structure of L proteins previously suggested by Poch etal. (22) could also be identified in the HeV L protein. A sequencecomparison of the most conserved domain (domain III) and the fourconserved motifs therein is shown in Fig. 1A. The C motif in domainIII of HeV L had a sequence of GDNE instead of GDNQ, a surprisingfinding in view of the fact that GDNQ is conserved among all NNSRNA virus L genes sequenced so far, the sole exception being theTPMV L protein (see Fig. 1B for a more detailed and expanded comparison).

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FIG. 1. (A) Alignment of four polymerase motifs (A to D) located within domain III of L proteins from selected Paramyxovirinae members. Residues identical in all viruses are shown as dots. Abbreviations: HeV, Hendra virus; TPMV, Tupaia paramyxovirus; MeV, measles virus; CDV, canine distemper virus; SeV, Sendai virus; PIV3, human parainfluenza virus type 3; NDV, Newcastle disease virus; MuV, mumps virus; SV5, simian virus 5. See Table 4 for GenBank accession numbers for the sequences used in the alignment. (B) A more extensive alignment of the motif C sequence to include viruses from all four families of the order Mononegavirales. The unique E residue in the GDNE sequence of HeV and TPMV L proteins is indicated by an asterisk. Abbreviations and GenBank accession numbers for viruses not listed above are as follows: RPV, rinderpest virus (Z30697); PIV2, human parainfluenza virus type 2 (X57559); RSV, respiratory syncytial virus (U39661); APV, avian paramyxovirus (U65312); RAV, rabies virus (M31046); VSV, vesicular stomatitis virus (J02428); MBGV, Marburg virus (Z12132); EBOV, Ebola virus (AF086833); BDV, Borna disease virus (U04608).

Phylogenetic analysis of the full-length L protein sequences or the domain III sequences produced very similar trees, indicatingthat the HeV L protein is most closely related to, but distinctfrom, viruses in the Morbillivirus and Respirovirus genera inthe subfamily Paramyxovirinae (data notshown).

Sequences of the 3' and 5' termini of the HeV genome. The genome-end sequences were determined using a combination of two different approaches, and the results are summarized inFig. 2A. The termini of the HeV RNA genome and anti-genome areidentical for the first 12 nt and 19 of the first 23 nt. A comparisonof the 3' leader sequences of selected Paramyxovirinae virusesis shown in Fig. 2B. Overall, the sequence of HeV is more closelyrelated to those of respiroviruses and morbilliviruses than rubulaviruses.However, HeV is unique in that it has a G residue at position4 in lieu of an A residue in all the other viruses. At positions5, 10, and 12, HeV resembles members of the Respirovirus genus(A, G, and G, respectively) and differs from viruses in the Morbillivirusgenus (G, A, and T, respectively). The converse is true at position11, where a G residue is shared by HeV and morbilliviruses whilerespiroviruses have an A residue there.

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FIG. 2. Alignment of genome end sequences. (A) Alignment of the 3' leader and 5' trailer sequences of HeV. (B) Alignment of 3' leader sequences of selected Paramyxovirinae members. The unique HeV residue at position 4 is indicated by an asterisk. The downward pointing triangle indicates the N gene transcription start site. Abbreviations are given in the Fig. 1 legend; SV41, simian virus 41 (GenBank accession no. X64275).

The HeV 3' leader sequence was 55 nt, a length identical to those of the 3' leader sequences of other members of the subfamilyParamyxovirinae (Fig. 2B). The 5' trailer sequence of HeV was33 nt. Unlike that of the 3' leader, the size of the 5' trailercan vary quite substantially within the subfamily (see Table 4).

Gene start, stop, and intergenic sequences. For members of the family Paramyxoviridae, transcription of individual genes is carried out by a stop-and-reinitiation mechanismthat is controlled by conserved transcriptional sequences at thegene borders. Sequence comparison analyses revealed that HeV issimilar to members of the Respirovirus and Morbillivirus generain having a conserved intergenic trinucleotide sequence, 3'-GAA-5'.The transcriptional start and stop signals of all HeV genes togetherwith the consensus sequences are shown in Table 3. Comparisonof the HeV consensus sequences with those of the respirovirusesand morbilliviruses suggests that while the consensus sequenceof HeV gene start signals is similar to the consensus sequencesof the start signals of both, the HeV gene stop signals are morelike those of respiroviruses.

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TABLE 3. Gene start, stop, and intergenic sequences

Rule of six and other genomic features. It has been suggested that Paramyxovirinae genomes are replicated efficiently only when they are a multiple of 6 nt in length,and this has been dubbed the "rule-of-six" (3). The genomelength of HeV (18,234 nt) is a multiple of 6 and does conformto this rule (Table 4). Also listed in Table 4 are the subunithexamer-phasing positions of the transcription initiation sitefor each of the six genes and the P gene-editing site from selectedrepresentative members of the subfamily Paramyxovirinae. Severalinteresting observations can be made. (i) Members of each of thethree existing genera seem to have conserved hexamer-phasing positionsfor most of the genes. (ii) HeV has a pattern that is significantlydifferent from that of any of the other members of the subfamily.(iii) Although phylogenetic analysis suggested relatedness ofTPMV and HeV (30), TPMV seems to be more closely related tomorbilliviruses with respect to the hexamer-phasing positions.

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TABLE 4. Comparison of genome properties of HeV and selected Paramyxovininae viruses

While the genome size of HeV is much larger than those of most other Paramyxoviridae members, the sizes of its encoded sixmajor proteins are very similar to those of others in the familywith the exception of the P protein, which is approximately 100aa longer (33). The increase in genome size is mainly due tothe expansion of UTRs, especially at the 3' end of the mRNA withthe exception of the L gene (Fig. 3). This has resulted in a significantdrop in the coding percentage from an average of approximately92% for known Paramyxovirinae viruses to 82.1% for HeV. A similarobservation has been made for TPMV following the completion ofsequencing of the whole genome. Filoviruses are a further exampleof NNS viruses that have a low coding percentage, 71.6% for Ebolavirus and 76.5% for Marburg virus. On the other hand, the smallgenome of Borna disease virus has a very high coding percentage,95.2%.

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FIG. 3. Genome structure and size comparison of selected members from the four families within the order Mononegavirales. Genome size (in nucleotides) is given in parentheses for each virus. The sizes are relative to that of the Ebola virus. Only genes coding for major structural proteins are shown, using the following functional grouping: nucleocapsid proteins (solid box), proteins associated with RNA polymerase and/or ribonucleoprotein complex (shaded box), matrix proteins (hatched box), and membrane proteins (open box). See the Fig. 1 legend for GenBank accession numbers.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The genome structure of HeV resembles that of other Paramyxovirinae members in having six genes in the order 3'-N-P/V/C-M-F-G-L-5'.The size of each gene product is similar to that of other virusesin the subfamily with the exception of the P protein, which isapproximately 100 aa longer than the longest P protein previouslycharacterized (33). Analyses of the protein sequences of thefirst five genes strongly suggest that HeV represents a new evolutionarylineage within the subfamily Paramyxovirinae with a closer relationshipto members of the Respirovirus and Morbillivirus genera than theRubulavirus genus (10, 33, 35, 36). This is corroboratedby the present study of the L gene sequence. RNA polymerase (L)genes of NNS RNA viruses have been considered a reliable targetfor phylogenetic analysis due to their high degree of conservationduring evolution (22). The size, sequence, and domain structureof the HeV L protein are very similar to those of other virusesin the subfamily. Extensive phylogenetic analyses of both full-lengthL protein and the more conserved domain III sequences confirmedthat HeV is a member of the subfamily Paramyxovirinae and is moreclosely related to morbilliviruses and respiroviruses (data notpresented).

However, the L protein of HeV and TPMV differs from other NNS virus L proteins in one important respect. The 4-aa sequenceGDNQ that is absolutely conserved among all known NNS virus Lgenes, from the smallest genome of Borna disease virus to thelargest genome of Marburg virus, is replaced in these new virusesby GDNE (Fig. 1). This sequence resides in the highly conservedC motif of domain III of NNS virus RNA polymerases and is believedto be the core polymerase motif in which the GD dipeptide residesprecisely within a $beta$ -turn- $beta$ structure (22). The functional importanceof the GDNQ sequence in the L protein has been examined experimentallyfor rabies virus and vesicular stomatitis virus (VSV). Changingthe rabies virus L protein GDN sequence to GDD (the motif sharedby most positive-strand RNA viruses) or SDD (the motif observedamong segmented negative-strand RNA viruses) completely abolishedRNA polymerase activity (28). Replacement of GDNQ in rabiesvirus by GDNE generated a mutant L protein that retained lessthan 1% of wild-type RNA polymerase activity. In the case of theVSV L protein, changing GDN to GDD did not completely inactivatethe RNA polymerase but reduced its activity by 73%. However, alterationof GDNQ to GDNN reduced activity by more than 95% (29). Thesestudies suggested that the invariant GDNQ sequence is optimalfor RNA polymerase activity in the order Mononegavirales and indicatedthat the effect of mutation in the region varies from virus tovirus. Following the establishment of an HeV reverse geneticssystem, it will be interesting to determine whether mutation ofGDNE to the more conserved GDNQ will have any effect on HeV RNApolymeraseactivity.

In the genus Morbillivirus, the length of the 5' UTR for the L gene is 21 nt. In the genus Respirovirus, this varies from22 nt for human parainfluenza virus type 3 to 28 nt for Sendaivirus. The HeV L gene has a 5' UTR of 154 nt, which is the longestto be found within the subfamily Paramyxovirinae. The 3' UTR ofthe HeV L gene is 67 nt, which is similar to those of morbillivirusL genes (Table 2). It is interesting to note that the L geneis the only gene in the HeV genome that does not have a longer3' UTR than other Paramyxovirinae members. In that regard, itis also interesting to point out that the 5' UTR of the HeV Ngene was similar to those of other Paramyxovirinae members (36).Considering the vast variation in the lengths of UTRs for internalHeV genes (10, 33, 35, 36), it is tempting to suggestthat there might be selective pressure to maintain the sizes ofnot only the genome leader and trailer sequences in HeV (see below)but also the genome end proximal UTRs, i.e., the 5' UTR of theN gene and the 3' UTR of the Lgene.

The genome terminal sequences of paramyxoviruses are highly conserved, and there is complementarity between the 3'- and 5'-terminalsequences. These conserved terminal sequences, especially thefirst 12 nt, are thought to contain the genome and antigenomepromoters and are largely genus specific (2, 15). This featurehas been used as an important criterion in classification of theParamyxoviridae. For example, in a recent analysis, the differencebetween the genome-end sequences of NDV and other members of thegenus Rubulavirus has been cited as one of the main reasons forreclassification of NDV in a separate genus within the Paramyxovirinae(7). In the case of HeV, the difference between its genomeend sequences and those of other subfamily members is obviousand significant, especially the presence of a G residue at position4 in lieu of the A residue found in all other members of the subfamily.On the other hand, the size of the HeV 3' leader sequence, 55nt, is identical to those found for all members of the subfamilyParamyxovirinae, a fact consistent with the placing of HeV withinthe subfamily based on phylogenetic analyses. The length of the5' trailer sequence varies significantly within the subfamily,with TPMV having the longest at 590 nt and simian virus 41 (SV41)the shortest at 20 nt. In general, rubulaviruses have a shorter5' trailer sequence (20 to 32 nt), whereas morbilliviruses andrespiroviruses tend to have slightly longer sequences of 41 to45 and 45 to 58 nt, respectively. For HeV, the 5' trailer is 33nt, which is shorter than those of morbilliviruses andrespiroviruses.

Members of the family Paramyxoviridae not only have highly conserved genome end sequences for replication and transcriptionbut also have highly conserved transcription start and stop sequencesat each gene boundary (2, 15). For the Respirovirus and Morbillivirusgenera, the nontranscribed intergenic sequence that is found notonly between genes but also before the N and after the L genesis 3 nt in length. Its sequence, 3'-GAA-5' (or 5'-CTT-3' in theantigenome), is conserved for most, but not all, of the six genesof viruses within these genera. HeV is the first virus to be sequencedthat has the identical CTT sequence in all seven positions ofa six-transcription-unit genome (Table 3). In morbillivirusesand respiroviruses, at least one "imperfect" intergenic sequencehas been found in each of the viruses sequenced so far. Theseinclude trinucleotide sequences AAA, GTA, GGG, GCA, GTT, and TTT,and they are mainly located toward the 3' end of the antigenome,i.e., at the end of the H (HN) gene or L gene (14), with theexception of Sendai virus, which has a TTT sequence before theN gene (Fig. 2B). The gene start and stop signals for the sixHeV transcription units are also more conserved than their morbillivirusand respirovirus counterparts. Whether this near-perfect conservationof transcription signals represents a more ancient or modern configurationremains to be seen. A close examination of the complete genomesequence of TPMV, which became available only very recently (GenBankaccession no. AF079780), indicated that TPMV also has perfect5'-CTT-3' intergenic sequences at all of the seven positions.Together with the larger genome sizes (17,904 nt for TPMV and18,234 nt for HeV) and the unusual sequence GDNE at the putativecatalytic site of their L proteins, this makes HeV and TPMV uniqueamong Paramyxovirinae genomes that have been completely sequenced.Whether these unique features, i.e., perfect intergenic sequencesand the GDNE sequence of L protein, are interrelated and commonto all large-genome paramyxoviruses remains to beseen.

The template for paramyxovirus RNA synthesis is not naked RNA but the helical ribonucleoprotein core of the virus, a structurein which nucleotide hexamers are believed to be associated withindividual nucleocapsid (N) protein molecules (14). As a consequence,many Paramyxoviridae members have a genome length that is a multipleof 6 nt. Moreover, it has been shown that these genomes are effectivelyreplicated only when they are a multiple of 6 nt (14). In addition,it has been found that, within a genus, the transcription startsite for each gene tends to be conserved in relation to the hexamer-phasingposition as shown in Table 4 (7, 14). While the conservationof genome length in multiples of 6 nt may have a functional advantage,the functional role for a conserved hexamer-phasing position foreach gene is less obvious. Nevertheless, this may serve as anadditional molecular marker in studying virus evolution and theclassification of new viruses. The hexamer-phasing position ofthe HeV N gene is the same as that of cognate genes in the subfamilyas a result of the uniform length of 3' leader sequences withinthe subfamily. However, it is intriguing to find that HeV hasa hexamer-phasing pattern, "2, 3, 4, 4, 4, 3," that is significantlydifferent from those of other viruses in the subfamily. The hexamer-phasingpositions for the HeV P, A (G), and L genes are unique and notused by cognate genes in the subfamily. HeV is also unique inthat it uses hexamer-phasing position 5 for the P editing site.This position is not used by any other virus for either a P editingsite or transcription start site (14).

Previous studies based on RNA polymerase sequence analysis have revealed that, within the order Mononegavirales, the Filoviridaeare more closely related to viruses in the genera Respirovirusand Morbillivirus of the family Paramyxoviridae than to virusesin the family Rhabdoviridae (31). It is interesting that the3' leader sequence of Ebola virus is 55 nt, the same length asthat of all members of the subfamily Paramyxovirinae. The discoverythat HeV has a genome approximately 15% larger than other membersof the Paramyxoviridae family and that each HeV gene has longUTRs is also consistent with a possible evolutionary relationshipbetween the Paramyxovirinae and the Filoviridae. As pointed outpreviously, until the discovery of HeV, there had been a largegenome size gap of approximately 3 kb between the largest genomeof the Paramyxoviridae and the smallest genome of the Filoviridae.This gap has now been filled by the 18.2-kb genome of HeV. Itremains to be seen whether NiV will have a larger genome size.The recent completion of the 17.9-kb TPMV genome sequence hasprovided a further reduction in the size gap of paramyxovirusgenomes.

The data reported here on the L protein sequence, genome size, genome end sequences, hexamer-phasing positions, and gene startand stop signals, together with sequence and molecular featurespreviously reported for the other five genes (10, 33, 35,36), suggest that the newly identified HeV is a member of thesubfamily Paramyxovirinae. The data also demonstrate a clear needfor the creation of a separate genus within the subfamily to accommodatethe many significant differences between HeV and other existingmembers of the Paramyxovirinae. The name Henipavirus is here proposedfor a new genus that would include HeV as the type species andNiV as the second member of the genus. Although the complete genomestructure of NiV is not yet available, the strong antigenic cross-reactivitybetween NiV and HeV (5) and high sequence homology for theirN, P, M, F, and G genes (12) suggest that HeV and NiV are veryclosely relatedviruses.

Identification and characterization of HeV and related new viruses is important not only because a number of them are lethalto humans and/or domestic animals but also because of the insightsthey may provide into virus evolution. The pattern of genome organization,the correlation between genome size and virus family, and thelack of recombination suggest that virus families in the orderMononegavirales have evolved by expansion or deletion of UTRsand by gene duplication, rather than by introduction of geneticinformation from outside (25). In this regard, the exceptionallylarge genome of HeV reported here represents an important linkin the evolution of Mononegavirales viruses. It is interestingthat an emerging virus with a high profile due to its lethal infectionof humans and a variety of animals has also significantly expandedthe viral diversity within the Paramyxoviridae, which has raisedmore questions about the nature of virusevolution.

	ACKNOWLEDGMENTS

We thank Kaylene Selleck, Nadia Mayfield, and Gary Beddome for technicalassistance.

This work was supported in part by a grant from the National Health and Medical Research Council ofAustralia.

	FOOTNOTES

^* Corresponding author. Mailing address: CSIRO Livestock Industries, Australian Animal Health Laboratory, PO Bag 24, Geelong,Victoria 3220, Australia. Phone: 61-3-52275121. Fax: 61-3-52275555.E-mail: linfa.wang{at}li.csiro.au.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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J. Bacteriol.	Mol. Cell. Biol.	Microbiol. Mol. Biol. Rev.

Clin. Vaccine Immunol.	ALL ASM JOURNALS

1.	Allworth, A., K. Murray, and J. Morgan. 1996. A human case of encephalitis due to a lyssavirus recently identified in fruit bats. Commun. Dis. Intellig. 20:504.
2.	Bellini, W. J., P. A. Rota, and L. J. Anderson. 1998. Paramyxoviruses, p. 435-461. In L. Collier, A. Balows, and M. Sussman (ed.), Microbiology and microbial infections, vol. 1. Arnold, London, England.
3.	Calain, P., and L. Roux. 1993. The rule of six, a basic feature for efficient replication of Sendai virus defective interfering RNA. J. Virol. 67:4822-4830[Abstract/Free Full Text].
4.	Chant, K., R. Chan, M. Smith, D. E. Dwyer, and P. Kirkland. 1998. Probable human infection with a newly described virus in the family Paramyxoviridae. Emerg. Infect. Dis. 4:273-275[Medline].
5.	Chua, K. B., W. J. Bellini, P. A. Rota, B. H. Harcourt, A. Tamin, S. K. Lam, T. G. Ksiazek, P. E. Rollin, S. R. Zaki, W. J. Shieh, C. S. Goldsmith, J. T. Roehrig, B. Eaton, A. R. Gould, J. Olson, H. Field, P. Daniels, A. E. Ling, C. J. Peters, L. J. Anderson, and B. W. J. Mahy. 2000. Nipah virus, a newly emergent deadly praramyxovirus. Science 288:1432-1435[Abstract/Free Full Text].
6.	Chua, K. B., K. J. Joh, K. T. Wong, A. Kamarulzaman, P. S. K. Tan, T. G. Ksiazek, S. R. Zaki, G. Paul, S. K. Lam, and C. T. Tan. 1999. Fatal encephalitis due to Nipah virus among pig-farmers in Malaysia. Lancet 354:1257-1259[CrossRef][Medline].
7.	de Leeuw, O., and B. Peeters. 1999. Complete nucleotide sequence of Newcastle disease virus: evidence for the existence of a new genus within the subfamily Paramyxoviridae. J. Gen. Virol. 80:131-136[Abstract].
8.	Field, H., J. M. Yob, C. Morrissy, and P. Selleck. 1999. Nipah virus in Malaysia $---$ preliminary wildlife surveillance, p. 187. In Proceedings of the XIth International Congress of Virology, Sydney, Australia.
9.	Fraser, G. C., P. T. Hooper, R. A. Lunt, A. R. Gould, L. J. Gleeson, A. D. Hyattt, G. M. Russell, and J. A. Kattenbelt. 1996. Encephalitis caused by a lyssavirus in fruit bats in Australia. Emerg. Infect. Dis. 2:327-331[Medline].
10.	Gould, A. R. 1996. Comparison of the deduced matrix and fusion protein sequences of equine morbillivirus with cognate genes of the Paramyxoviridae. Virus Res. 43:17-31[CrossRef][Medline].
11.	Halpin, K., P. Young, and H. Field. 1996. Identification of likely natural hosts for equine morbillivirus. Commun. Dis. Intellig. 20:476.
12.	Harcourt, B. H., A. Tamin, T. G. Ksiazek, P. E. Rollin, L. J. Anderson, W. J. Bellini, and P. A. Rota. 2000. Molecular characterization of Nipah virus, a newly emergent paramyxovirus. Virology 271:334-349[CrossRef][Medline].
13.	Hooper, P. T., A. R. Gould, A. D. Hyatt, M. A. Braun, J. A. Kattenbelt, S. G. Hengstberger, and H. A. Westbury. 2000. Identification and molecular characterisation of Hendra virus in a horse in Queensland. Aust. Vet. J. 78:281-282[Medline].
14.	Kolakofsky, D., T. Pelet, D. Garcin, S. Hausmann, J. Curran, and L. Roux. 1998. Paramyxovirus RNA synthesis and the requirement for hexamer genome length: the rule of six revisited. J. Virol. 72:891-899[Free Full Text].
15.	Lamb, R. A., and D. Kolakofsky. 1996. Paramyxoviridae: the viruses and their replication, p. 1177-1204. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed. Lippincott-Raven, Philadelphia, Pa.
16.	Mackenzie, J. S. 1999. Emerging viral diseases: an Australian perspective. Emerg. Infect. Dis. 5:1-8[Medline].
17.	Mayo, M. A., and C. R. Pringle. 1998. Virus taxonomy $---$ 1997. J. Gen. Virol. 79:649-657[Medline].
18.	Moritz, R. L., J. Eddes, H. Ji, G. E. Reid, and R. J. Simpson. 1995. Rapid separation of proteins and peptides using conventional silica-based supports: identification of 2-D gel proteins following in-gel proteolysis, p. 311-319. In J. W. Crabb (ed.), Techniques in protein chemistry, vol. VI. Academic Press, New York, N.Y.
19.	Murray, K., P. Selleck, P. Hooper, A. Hyatt, A. Gould, L. Gleeson, H. Westbury, L. Hiley, L. Selvey, and B. Rodwell. 1995. A morbillivirus that caused fatal disease in horses and humans. Science 268:94-97[Abstract/Free Full Text].
20.	O'Sullivan, J. D., A. M. Allworth, D. L. Paterson, T. M. Snow, R. Boots, L. J. Gleeson, A. R. Gould, A. D. Hyatt, and J. Bradfield. 1997. Fatal encephalitis due to novel paramyxovirus transmitted from horses. Lancet 349:93-95[CrossRef][Medline].
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