Isolation and Characterization of a Hantavirus from Lemmus sibiricus: Evidence for Host Switch during Hantavirus Evolution

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Journal of Virology, July 1999, p. 5586-5592, Vol. 73, No. 7
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Isolation and Characterization of a Hantavirus from Lemmus sibiricus: Evidence for Host Switch during Hantavirus Evolution

Olli Vapalahti,¹^,^* Åke Lundkvist,² Vadim Fedorov,³ Christopher J. Conroy,⁴ Sirpa Hirvonen,¹ Angelina Plyusnina,¹ Kirill Nemirov,¹ Karl Fredga,³ Joseph A. Cook,⁴ Jukka Niemimaa,⁵ Asko Kaikusalo,⁵ Heikki Henttonen,⁵ Antti Vaheri,¹ and Alexander Plyusnin¹

Department of Virology, Haartman Institute, FIN-00014 University of Helsinki,¹ and Finnish Forest Research Institute, FIN-01301 Vantaa,⁵ Finland; Swedish Institute for Infectious Disease Control, SE-171 82 Stockholm, and Microbiology and Tumor Biology Center, Karolinska Institute, SE-171 77 Stockholm,² and Department of Genetics, University of Uppsala, S-75007 Uppsala,³ Sweden; and Department of Mammalogy, University of Alaska Museum, Fairbanks, Alaska 99775-6960⁴

Received 30 September 1998/Accepted 19 March 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results and Discussion References

A novel hantavirus, first detected in Siberian lemmings (Lemmus sibiricus) collected near the Topografov River in the TaymyrPeninsula, Siberia (A. Plyusnin et al., Lancet 347:1835-1836,1996), was isolated in Vero E6 cells and in laboratory-bred Norwegianlemmings (Lemmus lemmus). The virus, named Topografov virus (TOP),was most closely related to Khabarovsk virus (KBR) and Puumalaviruses (PUU). In a cross focus reduction neutralization test,anti-TOP Lemmus antisera showed titers at least fourfold higherwith TOP than with other hantaviruses; however, a rabbit anti-KBRantiserum neutralized TOP and KBR at the same titer. The TOP Msegment showed 77% nucleotide and 88% amino acid identity withKBR and 76% nucleotide and 82% amino acid identity with PUU. However,the homology between TOP and the KBR S segment was disproportionatelyhigher: 88% at the nucleotide level and 96% at the amino acidlevel. The 3' noncoding regions of KBR and the TOP S and M segmentswere alignable except for 113- and 58-nucleotide deletions inKBR. The phylogenetic relationships of TOP, KBR, and PUU and theirrespective rodent carriers suggest that an exceptional host switchtook place during the evolution of these viruses; while TOP andKBR are monophyletic, the respective rodent host species are onlydistantlyrelated.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results and Discussion References

The members of the genus Hantavirus, family Bunyaviridae, are each primarily carried by a different, specific rodent hostspecies. The phylogeny of the hantaviruses has been shown to mirrorthe relatedness of their respective carrier species, suggestingcoevolution of the viruses with their hosts (35). The permanenttransmission of hantavirus to another rodent species has beendocumented only once (27); permanent transmission between differentrodent genera has never been documented. However, temporary spilloverto secondary hosts, such as other rodent species or humans, wherehantaviruses can cause hemorrhagic fever with renal syndrome andhantavirus pulmonary syndrome, may occur (for a review, see references16, 23, 35, and 40). In northern Europe, the predominantpathogenic hantavirus is Puumala virus (PUU), carried by the bankvole Clethrionomys glareolus. Other known hantavirus carrier rodentson the Eurasian continent include species of Rattus, Apodemus,and Microtus.

Lemmings are arvicoline rodents inhabiting the Arctic tundra. Lemmus lemmus of Fennoscandia (the area comprising Norway, Sweden,Finland, and adjacent areas of Russia) is closely related to thewestern type Lemmus sibiricus, whose distribution extends to theTaymyr Peninsula in Russia to the east (Fig. 1). Together, thesetwo are genetically more distantly related to the central typeof L. sibiricus (found from the Lena to the Kolyma Rivers) andto the eastern type (found east of the Kolyma River and in Alaska),also known as Lemmus trimucronatus) (8). L. lemmus is wellknown for its drastic population fluctuations and mass migrations(12). The spring migration of lemmings during one peak populationyear, 1942, coincided with an outbreak of more than 1,000 casesof a mild hemorrhagic fever-like illness among Finnish and Germantroops stationed in Salla, Finland (14, 44).

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FIG. 1. Geographic origin of the infected wild rodents (localities indicated by arrows) and the geographical distribution of (i) L. lemmus and L. sibiricus western type (found west of the Lena River) (ii) L. sibiricus central type (found between the Lena and Kolyma Rivers), and (iii) L. sibiricus eastern type (or L. trimucronatus, found east of the Kolyma River) (8, 10). Localities from which lemming samples were analyzed are shown by dots. In addition, Finse, Norway, (origin of the lemming colony), and Salla, Finland (the site of a putative lemming-borne outbreak in 1942), are indicated.

The presence of hantaviral antigen in lemmings in Arctic Siberia has been previously reported (28). To screen for a hantavirusin lemmings, we obtained lemming liver samples that were collectedin several locations along the Siberian coast during the Swedish-RussianTundra Ecology Expedition of 1994 (Fig. 1).

Our aim was to isolate the hantavirus present in this evolutionarily distinct arvicoline rodent in cell culture and to characterizeit genetically and antigenically. When this was achieved, theisolated virus was found to have striking similarities to anotherhantavirus, Khabarovsk virus (KBR), isolated from an evolutionarilydistant arvicoline rodent species, Microtus fortis, in the Russianfar east (7, 13). This led us to further compare the phylogeneticrelationships between the hantavirus genomes from the carrierrodents and their mitochondrial DNAsequences.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results and Discussion References

Viruses. All hantavirus strains were propagated in a biosafety level 3 laboratory in Vero E6 cells cultivated in Eagle's minimal essentialmedium supplemented with 2% fetal calf serum, 2 mM L-glutamine,penicillin, and streptomycin. The following hantavirus strainswere used: Hantaan/76-118 (HTN) (17), Puumala/Sotkamo (PUU)(3, 41), Prospect Hill/PH-1 (PH) (18), KBR/MF-43 (KBR)(7, 13), Tula/M02V (TUL) (48), and Sin Nombre/CC107 (SN)(39).

Collection and screening of rodent samples. The lemming liver samples from Siberia were collected during the Swedish-Russian Tundra Ecology Expedition of 1994 (10).Altogether, 231 samples from 12 localities (Fig. 1) were screenedby immunoblotting for hantavirus N antigen with a rabbit antiserumraised against recombinant PUU N antigen (anti-GST-PUU-N2/3) (47).

Virus isolation and production of antisera. Isolation of hantavirus in Vero E6 cells was performed by inoculating diluted, homogenized lemming liver tissue (stored for2 years at $-$ 70°C) into Vero E6 cells and passaging the cells bytrypsinization and the addition of fresh cells (at a 1 to 3 ratioto the rest of the cells) every 3 weeks as described previously(48). The cells were checked by immunofluorescence assay (IFA)with monoclonal antibody (MAb) 1C12 (21) for hantavirus antigen.The isolated virus was purified by a sucrose gradient as describedbefore (48).

The same liver samples were inoculated subcutaneously and intranasally into laboratory-bred hantavirus antibody-negative L.lemmus lemmings from Finse, Norway. The inoculated lemmings werethen sacrificed 30 days later and checked for anti-PUU antibodiesby IFA and for N antigen by immunoblotting with a rabbit antiserumas described above. The generation of polyclonal antisera fora focus reduction neutralization test (FRNT) was achieved by theintranasal inoculation of New Zealand White rabbits as describedpreviously (30). In addition, the sera of experimentally infectedL. lemmus lemmings wereused.

Reverse transcription-PCR, cloning, and sequencing of viral sequences. RNA extraction (5) was done similarly for infected Vero E6 cell cultures and rodent samples. The entire S segment was amplifiedby using one primer and was cloned as described before (32,34). The M segment was amplified and cloned in three parts;for the L segment (nucleotides [nt] 181 to 514), a pair of nestedprimers was used (sequences are available upon request). For thisstudy, the KBR (13) total M segment sequence was also completed,and a partial L segment sequence of KBR and PH was determined.The PCR amplicons were separated in agarose gels and purifiedwith the QIAquick kit (Qiagen GmbH). Direct sequencing was performedwith an ABI Prism dye terminator sequencing kit (Perkin-ElmerApplied Biosystems Division [PE/ABI], Foster City, Calif.) accordingto the manufacturer's instructions, and reactions were run onan ABI 373 A sequencer (PE/ABI). Cloning of the PCR products wasdone with a PGEM-T cloning kit (Promega). Plasmids were purifiedwith either the Wizard Mini-preps kit (Promega) or the QIAprepkit (Qiagen GmbH) and sequenced either with Sequenase, version2.0 (United States Biochemicals), or automatically. In the lattercase, sequencing was performed with either an ABI Prism dye terminatoror ABI Prism M13F and M13R dye primer sequencing kit (PE/ABI).

Rodent sequences. Mitochondrial cytochrome b gene (cyt b) DNA sequences were either downloaded from GenBank or generated in the laboratory.The rodent data are part of a larger study on the evolution ofarvicoline genera and species of Microtus. They will be publishedin complete form elsewhere (6). Samples were derived from differentrodent species from various collections as follows (sample numberin parentheses). (i) Apodemus flavicollis (AF 3326), Clethrionomysglareolus (AF 3133), Clethrionomys rufocanus (AF 3783), L. sibiricus(AF 15478), L. trimucronatus (AF 4077), Microtus californicus(AF 15891), Microtus pennsylvanicus (AF 2511), and Peromyscusmaniculatus (AF 17750) samples were from the Alaska Frozen TissueCollection, University of Alaska Museum, Fairbanks; (ii) a Reithrodontomysmegalotis sample (812 bases, UAM 38139 [skin]) was from the Universityof Alaska Museum; and (iii) an M. fortis sample (MVZ 1524) wasfrom the Museum of Vertebrate Zoology, University of California,Berkeley. DNA was extracted from samples of heart or skin viaa modified salt method (25). Symmetric PCR (37) was used toamplify portions of the cyt b gene (Mus mitochondrial DNA, basepairs [bp] 14139 to 15282) (1) with standard cyt b primers(6, 42) and PCR protocols. Sequences for both strands weredetermined on an ABI 373a stretch DNA sequencer with a Prism dyeterminator kit (Fst-RR, 402119; Perkin-Elmer).

Phylogenetic analyses. The PHYLIP program package (9) was used to make 200 bootstrap replicates of the sequence data (Seqboot). Distance matriceswere calculated by using Kimura's two-parameter model (Dnadist)and analyzed by the Fitch-Margoliash tree-fitting algorithm (Fitch).The bootstrap support percentages of particular branching pointswere calculated from these trees (Consense). For comparison, existingsequence data were obtained fromGenBank.

The S segment sequences include KBR/MF-43 (GenBank accession no. U35255), PUU/Sotkamo (X61035), PUU/Vindeln/83-L20 (Z48586),PUU/Bashkiria/CG1820 (M32750), PUU/France/90-13 (U22423),PUU/Tobetsu (B010731), PUU/Udmurtia/894Cg/91 (Z21497), TUL/Moravia/5286Ma/94(Z48573), TUL/76Ma/87 (Z30941), PH/PH-1 (Z49098), IslaVista (ILV)/MC-SB-1 (U31534), SN/HlO (L25784), New York(NY)/RI-1 (U09488), El Moro Canyon (ELMC)/RM-97 (U11427),Laguna Negra (LN)/510B (AF005727), Rio Segundo (RIOS)/RMx-Costa-I(U18100), Rio Mamore (RIOM) (U52136), Bayou (BAY)/Louisiana(L36929), Black Creek Canal (BCC) (L39949), Seoul (SEO)/SR-11(M34882), HTN/76-118 (M146271), and Dobrava (DOB)/Slovenia(L41916).

The M segment sequences included PUU/Sotkamo (X61034), PUU/Vindeln/83-L20 (Z49214), PUU/Bashkiria/CG1820 (M29979),PUU/Kazan (Z84205), PUU/France90-13 (U22418), TUL/Moravia/5286Ma/94(Z66538), PH/PH-1 (Z55129), SN/Hl0 (L25783), NY/RI-1(U36801), ELMC/RM-97 (U26828), LN/510B (AF005728), BAY/Louisiana(L36930), BCC (L39950), SEO/SR-11 (M34881), HTN/76118(M14627), Dobrava (DOB) (L33685), and Thailand (THAI)/749(L08756). The L segment sequences included PUU/Sotkamo (Z66548),PUU/Bashkiria/CG1820 (M63194), SN/H10 (L37901), BCC (L39951),SEO/80-39 (X56492), and HTN/76-118 (X55901).

The rodent cyt b sequences were aligned by eye. The following rodent cyt-b sequences were downloaded from GenBank (full cytb sequence if not otherwise indicated): Calomys lepidus (801 bases,U03544), Microtus arvalis (U54488), Oligoryzomys microtis(801 bases, U58381), Oryzomys palustris (401 bases, L37388),Peromyscus leucopus (321 bases, X89790), and Rattus rattus(X14848). By using the PHYLIP program package (9), Kimuratwo-parameter distances (Dnadist) were analyzed by the Fitch-Margoliashtree-fitting algorithm (Fitch). Bootstrap percentages for 250iterations were calculated (Seqboot), and TreeMap software (31)was used to construct a "tanglegram" of murid rodents and associatedhantaviruses.

MAbs and IFA. A panel of MAbs (21, 24) and recombinant Fab fragments (38) was used in a standard IFA on acetone-fixed, hantavirus-infectedVero E6 cells (21).

FRNT. Endpoint titers of neutralizing antibodies were determined by FRNT (30). Dilutions of sera were mixed with an equal volumecontaining 30 to 70 focus-forming units of virus/100 µl. The mixturewas incubated for 1 h and subsequently inoculated onto confluentVero E6 cell monolayers in six-well plates. After adsorption for1 h, the wells were overlaid with a mixture of agarose and basalEagle's medium. Plates were incubated for 9 (HTN), 10 (KBR), or12 (PUU, PH, Topografov virus [TOP], TUL, and DOB) days. Virus-infectedcells were detected with hantavirus-specific polyclonal antisera,followed by peroxidase-labeled goat antibodies and a substrate.An 80% reduction in the number of foci was the criterion for virusneutralizationtiters.

HI test. A goose erythrocyte hemagglutination inhibition (HI) test was performed essentially as described previously (4). PUU-,TOP-, and KBR-infected Vero E6 cell culture supernatants (forTUL, a sucrose gradient peak fraction) treated with Tween 20-ether(1:1 ratio) were used as hemagglutination antigens with 3 hemagglutinationunits of antigen perwell.

Nucleotide sequence accession numbers. The TOP S, M, and partial L sequences are deposited in GenBank with accession no. AJ011646, AJ011647, and AJ011649,respectively; the KBR total M genome and partial L segment sequencesare deposited with accession no. AJ011648 and AJ011650,respectively; and the PH partial L sequence is deposited withaccession no. AJ011651.

	RESULTS AND DISCUSSION

Top Abstract Introduction Materials and Methods Results and Discussion References

Isolation of TOP. Altogether, 231 liver samples from Siberian lemmings (L. sibiricus), collected in 12 localities during the Swedish-RussianTundra Ecology Expedition of summer 1994, were screened for hantavirusantigen by immunoblotting; 6 specimens were positive. These animalswere among 61 collected from two localities (no. 8 and 10) onthe Taymyr Peninsula (Fig. 1) (33).

Each positive sample was injected into Norwegian lemmings (L. lemmus) originating from Finse, Norway. The virus was successfullypassaged in (four of six) laboratory lemmings, with the presenceof antigen in the lungs demonstrated by immunoblotting (four ofsix) and/or with the development of anti-PUU antibodies demonstratedby IFA (three of six). The lung tissues of antigen-positive lemmingswere used for RNA isolation, followed by reverse transcriptionand nested PCR. Initially, amplicons (354 bp in length) from theS genomic segment from two specimens were prepared. Subsequentsequencing revealed a previously unknown hantavirus genotype,named TOP according to its geographic origin, the area aroundthe Topografov River (33) (locality 10) (Fig. 1). Identicalsequences were also derived from the original lemmingsamples.

We also applied the same liver samples from wild lemmings onto Vero E6 cells without a prior passage in laboratory lemmings.After 9 weeks and two cell passages, four of six isolations wereclearly positive for hantavirus N antigen, including isolatesfrom individual samples from the two different locations. Oneof the isolates, designated TOP/Ls136V5/94 and originating fromlocality 10, was selected as the reference strain. The virus supernatantcould be passaged several times in Vero E6 cells, and the viruswas further purified by sucrose gradient ultracentrifugation;the viral peak was recovered at 42% (wt/vol) sucrose, where hantavirus-likeparticles could be distinguished by electron microscopy. TOP G1migrated more slowly in a sodium dodecyl sulfate-polyacrylamidegel than did PUU G1, whereas TOP G2 and N showed apparent molecularweights similar to those of PUU G2 and N (data notshown).

Antigenic properties. When studied with a panel of nucleocapsid protein-specific MAbs by IFA, TOP was found to be antigenically most closely relatedto KBR (Table 1). Two MAbs could be used to distinguish PUU fromTOP and KBR. The nucleocapsid proteins of TOP and KBR differedonly in reactivity to one anti-PUU MAb, 3H9, the epitope of whichhas been mapped to the most variable part of N, amino acids (aa)251 to 260 (20, 22). The reactivity of 3H9 with TOP was veryweak: aa 252 to 257 for TOP N were KPGAPA instead of KPGTPA inPUU and KBR, which most probably explains the different reactivity.We noted also that native SN was detected by two MAbs (1C8 and3C11) that were not reactive with recombinant SN nucleocapsidprotein (24) (Table 1).

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TABLE 1. Selected panel of nucleocapsid protein-specific MAbs and Fab fragments showing reactivities in an IFA

In a cross-FRNT, TOP was distinguishable from all other hantaviruses with at least a two-way fourfold titer difference (Table2) except for a one-way titer difference for KBR, as the anti-KBRrabbit antiserum neutralized KBR and TOP with the same titer (1:1,280).A similar pattern was obtained in an HI test.

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TABLE 2. Cross-FRNT and cross-HI comparison of TOP with other hantaviruses

Genetic properties. Sequencing of TOP S showed that the S segment consists of 1,953 nt and codes for a nucleocapsid protein of 433 aa and a putativenonstructural protein, NSs, of 90 aa. The sequence was most closelyrelated to that of KBR (82% nucleotide and 96% amino acid identityfor the S segment) and PUU (77% nucleotide and 87% amino acididentity) (Table 3). The 3' noncoding region (according to themessenger sense) of TOP S was alignable with that of KBR, showing77% nucleotide homology. However, the KBR S noncoding region hada deletion of 113 nt compared to the TOP S sequence.

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TABLE 3. S, M, and L segment nucleotide and amino acid identities of TOP with other hantaviruses

The M segment consisted of 3,735 nt and coded for a G1-G2 precursor of 1,142 aa. The M segment showed considerably more variationthan the S segment, but the pattern of relatedness to differenthantaviruses was the same, showing 77% nucleotide and 88% aminoacid identity between TOP and KBR and 76% nucleotide and 83% aminoacid identity between TOP and PUU (Table 3). Similarly to theS segment, a deletion of 55 nt was found in the 3' noncoding regionof KBR compared to TOP. The putative Asn-linked glycosylationsites in G1 and G2 were identical among TOP, PUU/Sotkamo, andKBR. The L segment sequence was analyzed from nt 181 to 514. Thisregion showed 81% nucleotide and 90% amino acid homology to theKBR L segment. Although the M segment tends to be the most variableof the hantavirus genome segments, the difference between theM and S segment amino acid homologies for TOP and KBR (88 and96%, respectively) is exceptionally high. While this could beexplained by reassortment, no sequence data currently availableon related viruses support this hypothesis. The discordant homologiesfor the two genome segments could mean that either (i) a recombinantvirus would have had better capabilities for a permanent hostswitch or (ii) after the host switch, an evolutionary pressurein a new host has generated more amino acid changes in the glycoproteinsthan in the nucleocapsidprotein.

TOP strain variation. TOP strains derived from the two localities (no. 8 and 10 [Fig. 1]) were analyzed by reverse transcription-PCR of a 354-ntfragment (nt 4 to 357) of the S segment and subsequent sequencing.Interestingly, in locality 8, two lineages showing 7.5% nucleotidedivergence cocirculated. The other lineage (represented by strain29) was surprisingly closely related (1% nucleotide divergence)to the TOP strains from locality 10 (no. 136 and 137). As localities8 and 10 are about 600 km apart, the lack of clear geographicclustering of genetic variants might reflect the dispersal capacityof lemmings (8).

Phylogenetic relationships of hantaviruses and respective rodent carriers. In the phylogenetic trees created for all three genome segments (Fig. 2), TOP was monophyletic with KBR. Furthermore, theTOP-KBR clade had a common origin with the PUU viruses with ahigh branching probability. A comparison of the phylogenetic treesof hantaviruses and their known carriers shows (Fig. 3) that coevolutionis a general rule (resulting in similar branching order for therodents and their respective hantaviruses). Also, a heuristicsearch for the best match between trees (31) suggested ninecospeciations. However, an evident host switch has occurred forthe ancestor of KBR from a PUU lineage, as KBR does not groupwith other Microtus-borne viruses but instead has a common nodeof origin, firstly with TOP and secondly with PUU, which are carriedby Lemmus and Clethrionomys, respectively. Another clear discrepancyin the arvicoline rodent phylogeny is that the branching of TOPfrom the PUU lineage is distal to the main Microtus-derived viruscluster (PH, TUL, and ILV), although the Clethrionomys and Microtusspecies are more closely related to each other and have a commonevolutionary origin (83% bootstrap support) compared to the moreancestral Lemmus (Fig. 3) (26). In fact, the branching positionof the common ancestor of KBR and TOP is not in line with thephylogeny with either of the host rodents.

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FIG. 2. Phylogenetic trees (PHYLIP) of hantavirus S (A), M (B), and partial L segments (C) (see Materials and Methods). Kimura two-parameter distances (Dnadist) were used to construct the Fitch-Margoliash tree (Fitch). Branching probabilities of >60% for different hantaviruses are indicated. PUU-Sotk, PUU-Sotkamo; TUL-02, Tula/M0ZV. Hantavirus strains are described in Materials and Methods.

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FIG. 3. Tanglegram constructed with TreeMap software (31), showing murid rodents and associated hantaviruses. The host tree on the left was generated from cyt b sequences, and the hantavirus S segment tree on the right was generated from S segment nucleotide sequences. Kimura two-parameter distances (Dnadist) were used to construct the Fitch-Margoliash tree (Fitch). Values indicate bootstrap percentages of >50% for 250 iterations (Seqboot). Trees were rerooted with Rattus rattus and SEO as outgroups. Hantavirus strains are described in Materials and Methods.

A hypothetical scenario for the host switch events might be that the ancestor of Clethrionomys, clearly after the divergenceof the rapidly radiating Microtus species approximately 1.5 millionyears ago (26), was the donor of an ancestral virus which becamethe common ancestor of both TOP and KBR. This ancestral virusbranch is separate from all PUU viruses from Japan to Belgium,which have a distinct, common node of origin. It is not certainif the ancestral virus was first transmitted to Lemmus; the longdeletions in the S and M segment 3' noncoding regions of KBR comparedto TOP suggest that TOP could represent a more ancestral virusthan KBR. However, the knowledge of the genetic diversity andgeographical distribution of TOP is limited. We screened morethan 400 L. lemmus samples from Fennoscandia and a total of 177lemmings from other locations in the Russian Arctic (Fig. 1) withoutfinding evidence of hantavirusantigen.

The geographic distributions of M. fortis and L. sibiricus do not overlap today (43), meaning that both species should permanentlycarry their respective viruses; i.e., TOP and KBR do not representspillover viruses. During the more than 3 million years that theClethrionomys-Microtus branch evolved from the common ancestorto Lemmus (36), the geographic ranges of the host rodent specieshave probably varied considerably, and the host switch(es) mayhave taken place, for example, in the southern ranges frequentedby the central L. sibiricusgroup.

Recent data on SN-like viruses of P. leucopus and P. maniculatus have shown that horizontal transmission between closely relatedspecies can occur (27). Another likely hantavirus host transfer(or possibly duplication) is suggested by the existence of Dobravavirus in both A. flavicollis and Apodemus agrarius in Europe (28a),while the latter carries the distinct Hantaan virus in far easternAsia. Data on South American hantaviruses and their host species,both of which have radiated rapidly (15, 19), are not in fullagreement with the coevolution in rodent host species (see, e.g.,the Laguna Negra virus, [Fig. 3]) (29). In the cases of TOPand KBR, while the sequence of events remains unclear, these arethe first clear indications that a hantavirus host switch eventcan indeed occur among more distantly related rodent species andeven between different rodent genera. Yet a host switch seemsto be a rare event, and cospeciation remains the rule. An analogyto the phylogeny of rodent carriers can be drawn, for example,with Arenaviridae (2) and even with some ectoparasites suchas lice (11), which show cospeciation with rodents and occasionalhost switches, resulting in new adaptivepeaks.

The taxonomic relationships of TOP and KBR are of special interest. If our hypothesis about a horizontal transmission, orhost switch, during evolution of these viruses is correct, itseems logical to assume that TOP and KBR are still radiating fromeach other. Ongoing radiation by the two viruses could be reflectedby different degrees of diversity for the M and S segments ofTOP and KBR. Nevertheless, based on an analysis of the combinationof properties of TOP and KBR, we believe that TOP and KBR fulfillthe criteria for demarcation (45) and should thus be considereddistinct virus species. The strongest argument for such a conclusionis that TOP and KBR have clearly distinct host species in whichthey are constantly maintained. The identification of additionalsequences from related hantaviruses might shed light on the originand relatedness of these viruses. For example, another hantavirusidentified from M. fortis in the Russian far east, Vladivostok,seems at least as divergent from KBR as TOP is (15a).

Is TOP a pathogen? We screened serum samples of World War II veterans who had been stationed in Salla, Finland, during the putative lemming-bornehantavirus outbreak of 1942 for hantavirus antibodies. While hantavirusantibodies were found in one-third of the samples, no differencein reactivity or antibody titers could be demonstrated betweenTOP, PUU, and KBR antigens by FRNT or with truncated recombinantantigens in an enzyme immunoassay (data not shown). However, similarresults were also found in samples from people with decades-oldPUU immunity who had no association with lemmings. It remainsto be determined whether a hantavirus actually circulates in lemmingsin Fennoscandia and if TOP can be transmitted to humans. However,it is possible that the outbreak of 1942 was caused by a hantaviruscarried by lemmings, since (i) the clinical symptoms mimickedthose later described for nephropathia epidemica, including highfever, acute renal failure, and, occasionally, myopia (14, 44);(ii) the year 1942 coincided with a mass migration of lemmingsin the region; and (iii) the incidence of the disease peaked inMay and June 1942, which coincides with the lemming spring migrationand contrasts with the epidemiology of the Clethrionomys-bornedisease, which normally peaks in November or December in Fennoscandia(46). As the population density of lemmings fluctuates strongly,it may be that only during occasional peak years do rodent densitiesreach the threshold necessary for the virus to spreadefficiently.

	ACKNOWLEDGMENTS

We thank Carl-Henrik von Bonsdorff and Anssi Mörttinen for electron micrographs and Tytti Manni, Leena Kostamovaara, andMari Gilljam for expert technical assistance. We thank Brian Hjellefor sharing primer sequences that were used for the initial detectionof the TOP S segment in lemming samples. Hiroaki Kariwa is acknowledgedfor sharing his data on Vladivostok virus and Stuart Nichol forhelpful discussions and for sharing the complete sequence of theKBR S segment and a manuscript beforepublication.

This work was supported by grants from the Wilhelm Stockmann Foundation, the Sigrid Jusélius Foundation, the European Commission(BMH4-CT97-2499), and the Swedish Medical Research Council (12177and12642).

	FOOTNOTES

^* Corresponding author. Mailing address: Haartman Institute, Dept. of Virology, P.O.B. 21, FIN-00014 University of Helsinki,Finland. Phone: 358-9-191 26486. Fax: 358-9-191 26491. E-mail:Olli.Vapalahti{at}helsinki.fi.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References

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3. Brummer-Korvenkontio, M., H. Henttonen, and A. Vaheri. 1982. Hemorrhagic fever with renal syndrome in Finland: ecology and virology of nephropathia epidemica. Scand. J. Infect. Dis. Suppl. 36:S88-S91.

4. Brummer-Korvenkontio, M., T. Manni, S. Ukkonen, and A. Vaheri. 1986. Detection of hemagglutination-inhibiting antibodies in patients with nephropathia epidemica and Korean hemorrhagic fever by using Puumala virus cell culture antigen. J. Infect. Dis. 153:997-998[Medline]. (Letter.)

5. Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium-phenol-chloroform extraction. Anal. Biochem. 162:156-159[Medline].

6. Conroy, C. J., and J. A. Cook. MtDNA evidence for repeated pulses of speciation within arvicoline and murid rodents. J. Mamm. Evol., in press.

7. Dzagurova, T., E. Tkachenko, R. Slonova, L. Ivanov, E. Ivanidze, S. Markeshin, A. Dekonenko, B. Niklasson, and A. Lundkvist. 1995. Antigenic relationships of hantavirus strains analysed by monoclonal antibodies. Arch. Virol. 140:1763-1773[Medline].

8. Fedorov, V., A. Goropashnaya, G. H. Jarrell, and K. Fredga. 1999. Phylogeographic structure and mitochondrial DNA variation in true lemmings (Lemmus) from the Eurasian Arctic. Biol. J. Linn. Soc. 66:357-371.

9. Felsenstein, J. 1993. PHYLIP (Phylogeny Inference Package), version 3.5c. University of Washington, Seattle.

10. Fredga, K., V. Fedorov, H. Gelter, G. Jarrell, and C.-G. Thulin. 1994. Genetic studies in lemmings, p. 235-242. In E. Grönlund, and O. Melander (ed.), Swedish-Russian tundra ecology expedition '94. Swedish Polar Research Secretariat, Stockholm, Sweden.

11. Hafner, M. S., P. D. Sudman, F. X. Villablanca, T. A. Spradling, J. W. Demastes, and S. A. Nadler. 1994. Disparate rates of molecular evolution in cospeciating hosts and parasites. Science 265:1087-1090[Abstract/Free Full Text].

12. Henttonen, H., and A. Kaikusalo. 1993. Lemming movements, p. 157-186. In N. C. Stenseth, and R. A. Inns (ed.), The biology of lemmings. Academic Press, Inc., New York, N.Y.

13. Hörling, J., V. Chizhikov, Å. Lundkvist, M. Jonsson, L. Ivanov, A. Dekonenko, B. Niklasson, T. Dzagurova, C. J. Peters, E. Tkachenko, and S. T. Nichol. 1996. Khabarovsk virus: a phylogenetically and serologically distinct hantavirus isolated from Microtus fortis trapped in far-east Russia. J. Gen. Virol. 77:687-694[Abstract/Free Full Text].

14. Hortling, H. 1946. En epidemi av fältfäber (?) i finska Lappland. Nord. Med. 30:1001-1004.

15. Johnson, A. M., M. D. Bowen, T. G. Ksiazek, R. J. Williams, R. Bryan, J. Mills, C. J. Peters, and S. T. Nichol. 1997. Laguna Negra virus associated with HPS in western Paraguay and Bolivia. Virology 238:115-127[Medline].

15a. Kariwa, H. Personal communication.

16. Khan, A. S., T. G. Ksiazek, and C. J. Peters. 1996. Hantavirus pulmonary syndrome. Lancet 347:739-741[Medline].

17. Lee, H. W., P. W. Lee, and K. M. Johnson. 1978. Isolation of the etiologic agent of Korean hemorrhagic fever. J. Infect. Dis. 137:289-308.

18. Lee, P. W., H. L. Amyx, D. C. Gajdusek, R. T. Yanagihara, D. Goldgaber, and C. J. Gibbs, Jr. 1982. New hemorrhagic fever with renal syndrome-related virus in rodents in the United States. Lancet ii:1405. (Letter.)

19. Levis, S., S. Morzunov, J. Rowe, D. Enria, N. Pini, G. Calderon, M. Sabattini, and S. C. St. Jeor. 1998. Genetic diversity and epidemiology of hantaviruses in Argentina. J. Infect. Dis. 177:529-538[Medline].

20. Lundkvist, Å., S. Björsten, B. Niklasson, and N. Ahlborg. 1995. Mapping of B-cell determinants in the nucleocapsid protein of Puumala virus: definition of epitopes specific for acute immunoglobulin G recognition in humans. Clin. Diagn. Lab. Immunol. 2:82-86[Abstract].

21. Lundkvist, Å., A. Fatouros, and B. Niklasson. 1991. Antigenic variation of European haemorrhagic fever with renal syndrome virus strains characterized using bank vole monoclonal antibodies. J. Gen. Virol. 72:2097-2103[Abstract/Free Full Text].

22. Lundkvist, Å., H. Kallio-Kokko, K. Brus Sjölander, H. Lankinen, B. Niklasson, A. Vaheri, and O. Vapalahti. 1996. Characterization of Puumala virus nucleocapsid protein: identification of B-cell epitopes and domains involved in protective immunity. Virology 216:397-406[Medline].

23. Lundkvist, Å., and B. Niklasson. 1994. Haemorrhagic fever with renal syndrome and other hantavirus infections. Rev. Med. Virol. 4:177-184.

24. Lundkvist, Å., O. Vapalahti, A. Plyusnin, K. Brus Sjölander, B. Niklasson, and A. Vaheri. 1996. Characterization of Tula virus antigenic determinants defined by monoclonal antibodies raised against baculovirus-expressed nucleocapsid protein. Virus Res. 45:29-44[Medline].

25. Medrano, J., E. Aasen, and L. Sharrow. 1990. DNA extraction from nucleated red blood cells. BioTechniques 8:43.

26. Modi, W. S. 1996. Phylogenetic history of LINE-1 among arvicolid rodents. Mol. Biol. Evol. 13:633-641[Abstract].

27. Morzunov, S. P., J. E. Rowe, T. G. Ksiazek, C. J. Peters, S. C. St. Jeor, and S. T. Nichol. 1998. Genetic analysis of the diversity and origin of hantaviruses in Peromyscus leucopus mice in North America. J. Virol. 72:57-64[Abstract/Free Full Text].

28. Myasnikov, Y. A., N. S. Apekina, A. P. Zuevskii, A. V. Khitrin, and A. D. Bernshtein. 1992. The disposition of natural foci of hemorrhagic fever with renal syndrome in different landscape areas of Tyumen Province. Vopr. Virusol. 37:161-165[Medline]. (In Russian.)

28a. Nemirov, K., O. Vapalahti, Å. Lundkvist, V. Vasilenko, I. Golovljova, A. Plyusnina, J. Niemimaa, J. Laakkonen, H. henttonen, A. Vaheri, A. Plyusnin. 1999. Isolation and characterisation of Dobrava hantavirus carried by the striped field mouse (Apodemus agrarius) in Estonia. J. Gen. Virol. 80:371-379.

29. Nichol, S. T. Genetic analysis of hantaviruses and their host relationships. In J. F. Saluzz and B. Dodet (ed.), Factors in the emergence and control of rodent-borne viral diseases (hantaviruses and arenaviruses), in press. Elsevier, Paris, France.

30. Niklasson, B., M. Jonsson, Å. Lundkvist, J. Horling, and E. Tkachenko. 1991. Comparison of European isolates of viruses causing hemorrhagic fever with renal syndrome by a neutralization test. Am. J. Trop. Med. Hyg. 45:660-665.

31. Page, R. D. M. 1997. Tree map, version 1.0c. University of Glasgow, Glasgow, Scotland.

32. Plyusnin, A., O. Vapalahti, H. Lankinen, H. Lehväslaiho, N. Apekina, Y. Myasnikov, H. Kallio-Kokko, H. Henttonen, Å. Lundkvist, M. Brummer-Korvenkontio, I. Gavrilovskaya, and A. Vaheri. 1994. Tula virus: a newly detected hantavirus carried by European common voles. J. Virol. 68:7833-7839[Abstract/Free Full Text].

33. Plyusnin, A., O. Vapalahti, Å. Lundkvist, H. Henttonen, and A. Vaheri. 1996. Newly recognized hantavirus in Siberian lemmings. Lancet 347:1835-1836[Medline].

34. Plyusnin, A., O. Vapalahti, K. Ulfves, H. Lehvaslaiho, N. Apekina, I. Gavrilovskaya, V. Blinov, and A. Vaheri. 1994. Sequences of wild Puumala virus genes show a correlation of genetic variation with geographic origin of the strains. J. Gen. Virol. 75:405-409[Abstract/Free Full Text].

35. Plyusnin, A., O. Vapalahti, and A. Vaheri. 1996. Hantaviruses: genome structure, expression and evolution. J. Gen. Virol. 77:2677-2687[Abstract/Free Full Text].

36. Repenning, C., O. Fejfar, and W.-D. Heinrich. 1990. Arvicolid rodent biochronology of the northern hemisphere, p. 385-418. In International Symposium on Evolution, Phylogeny, and Biostratigraphy of Arvicolids (Rodentia, Mammalia).Pfeil-Verlag, Prague, Czechoslovakia.

37. Saiki, R., D. Gelfand, S. Stoffel, S. Scharf, R. Higuchi, G. Horn, K. Mullis, and H. Erlich. 1981. Primer-directed enzymatic amplification of DNA with a thermostable DNA polymerase. Science 239:487-491.

38. Salonen, E.-M., P. Parren, Y. Graus, Å. Lundkvist, P. Fisicaro, O. Vapalahti, H. Kallio-Kokko, A. Vaheri, and D. Burton. 1998. Human recombinant Puumala virus antibodies: cross reaction with other hantaviruses and use in diagnostics. J. Gen. Virol. 79:667-671[Abstract].

39. Schmaljohn, A. L., D. Li, D. L. Negley, D. S. Bressler, M. J. Turell, G. W. Korch, M. S. Ascher, and C. S. Schmaljohn. 1995. Isolation and initial characterization of a newfound hantavirus from California. Virology 206:963-972[Medline].

40. Schmaljohn, C., and B. Hjelle. 1997. Hantaviruses: a global disease problem. Emerg. Infect. Dis. 3:95-104[Medline].

41. Schmaljohn, C. S., S. E. Hasty, J. M. Dalrymple, J. W. LeDuc, H. W. Lee, C.-H. von Bonsdorff, M. Brummer-Korvenkontio, A. Vaheri, T. F. Tsai, H. L. Regnery, D. Goldgaber, and P. W. Lee. 1985. Antigenic and genetic properties of viruses linked to hemorrhagic fever with renal syndrome. Science 227:1041-1044[Abstract/Free Full Text].

42. Smith, M. F., and J. L. Patton. 1993. The diversification of South American murid rodents: evidence from mitochondrial DNA sequence data for the akodontine tribe. Biol. J. Linn. Soc. 50:149-177.

43. Stenseth, N. C., and R. A. Ims (ed.). 1993. The biology of lemmings. Academic Press, Inc., New York, N.Y.

44. Stuhlfault, K. 1943. Bericht über ein neues schlammfieberähnliches Krankenheitsbild bei Deutschen Truppen in Lappland. Dtsch. Med. Wochenschr. 69:439-443, 474-477.

45. Van Regenmortel, M. H. V., D. H. L. Bishop, C. M. Fauquet, M. A. Mayo, J. Maniloff, and C. H. Calisher. 1997. Guidelines to the demarcation of virus species. Arch. Virol. 142:1505-1528[Medline].

46. Vapalahti, K., M. Paunio, A. Vaheri, and O. Vapalahti. Epidemiology of Puumala virus infections in Finland: increased risk for farmers. Am. J. Epidemiol., in press.

47. Vapalahti, O., H. Kallio-Kokko, A. Närvänen, I. Julkunen, Å. Lundkvist, A. Plyusnin, H. Lehväslaiho, M. Brummer-Korvenkontio, A. Vaheri, and H. Lankinen. 1995. Human B-cell epitopes of Puumala virus nucleocapsid protein, the major antigen in early serological response. J. Med. Virol. 46:293-303[Medline].

48. Vapalahti, O., Å. Lundkvist, S. K. J. Kukkonen, Y. Cheng, M. Gilljam, M. Kanerva, T. Manni, M. Pejcoch, J. Niemimaa, A. Kaikusalo, A. Henttonen, A. Vaheri, and A. Plyusnin. 1996. Isolation and characterization of Tula virus, a distinct serotype in the genus Hantavirus, family Bunyaviridae. J. Gen. Virol. 77:3063-3067[Abstract/Free Full Text].

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1.	Bibb, M. J., R. A. Van Etten, C. T. Wright, M. W. Walberg, and D. Clayton. 1981. Sequence and gene organization of mouse mitochondrial DNA. Cell 26:167-180[Medline].
2.	Bowen, M., C. J. Peters, J. M. Mills, and S. T. Nichols. 1996. Oliveros virus: a novel arenavirus from Argentina. Virology 217:362-366[Medline].
3.	Brummer-Korvenkontio, M., H. Henttonen, and A. Vaheri. 1982. Hemorrhagic fever with renal syndrome in Finland: ecology and virology of nephropathia epidemica. Scand. J. Infect. Dis. Suppl. 36:S88-S91.
4.	Brummer-Korvenkontio, M., T. Manni, S. Ukkonen, and A. Vaheri. 1986. Detection of hemagglutination-inhibiting antibodies in patients with nephropathia epidemica and Korean hemorrhagic fever by using Puumala virus cell culture antigen. J. Infect. Dis. 153:997-998[Medline]. (Letter.)
5.	Chomczynski, P., and N. Sacchi. 1987. Single-step method of RNA isolation by acid guanidinium-phenol-chloroform extraction. Anal. Biochem. 162:156-159[Medline].
6.	Conroy, C. J., and J. A. Cook. MtDNA evidence for repeated pulses of speciation within arvicoline and murid rodents. J. Mamm. Evol., in press.
7.	Dzagurova, T., E. Tkachenko, R. Slonova, L. Ivanov, E. Ivanidze, S. Markeshin, A. Dekonenko, B. Niklasson, and A. Lundkvist. 1995. Antigenic relationships of hantavirus strains analysed by monoclonal antibodies. Arch. Virol. 140:1763-1773[Medline].
8.	Fedorov, V., A. Goropashnaya, G. H. Jarrell, and K. Fredga. 1999. Phylogeographic structure and mitochondrial DNA variation in true lemmings (Lemmus) from the Eurasian Arctic. Biol. J. Linn. Soc. 66:357-371.
9.	Felsenstein, J. 1993. PHYLIP (Phylogeny Inference Package), version 3.5c. University of Washington, Seattle.
10.	Fredga, K., V. Fedorov, H. Gelter, G. Jarrell, and C.-G. Thulin. 1994. Genetic studies in lemmings, p. 235-242. In E. Grönlund, and O. Melander (ed.), Swedish-Russian tundra ecology expedition '94. Swedish Polar Research Secretariat, Stockholm, Sweden.
11.	Hafner, M. S., P. D. Sudman, F. X. Villablanca, T. A. Spradling, J. W. Demastes, and S. A. Nadler. 1994. Disparate rates of molecular evolution in cospeciating hosts and parasites. Science 265:1087-1090[Abstract/Free Full Text].
12.	Henttonen, H., and A. Kaikusalo. 1993. Lemming movements, p. 157-186. In N. C. Stenseth, and R. A. Inns (ed.), The biology of lemmings. Academic Press, Inc., New York, N.Y.
13.	Hörling, J., V. Chizhikov, Å. Lundkvist, M. Jonsson, L. Ivanov, A. Dekonenko, B. Niklasson, T. Dzagurova, C. J. Peters, E. Tkachenko, and S. T. Nichol. 1996. Khabarovsk virus: a phylogenetically and serologically distinct hantavirus isolated from Microtus fortis trapped in far-east Russia. J. Gen. Virol. 77:687-694[Abstract/Free Full Text].
14.	Hortling, H. 1946. En epidemi av fältfäber (?) i finska Lappland. Nord. Med. 30:1001-1004.
15.	Johnson, A. M., M. D. Bowen, T. G. Ksiazek, R. J. Williams, R. Bryan, J. Mills, C. J. Peters, and S. T. Nichol. 1997. Laguna Negra virus associated with HPS in western Paraguay and Bolivia. Virology 238:115-127[Medline].
15a.	Kariwa, H. Personal communication.
16.	Khan, A. S., T. G. Ksiazek, and C. J. Peters. 1996. Hantavirus pulmonary syndrome. Lancet 347:739-741[Medline].
17.	Lee, H. W., P. W. Lee, and K. M. Johnson. 1978. Isolation of the etiologic agent of Korean hemorrhagic fever. J. Infect. Dis. 137:289-308.
18.	Lee, P. W., H. L. Amyx, D. C. Gajdusek, R. T. Yanagihara, D. Goldgaber, and C. J. Gibbs, Jr. 1982. New hemorrhagic fever with renal syndrome-related virus in rodents in the United States. Lancet ii:1405. (Letter.)
19.	Levis, S., S. Morzunov, J. Rowe, D. Enria, N. Pini, G. Calderon, M. Sabattini, and S. C. St. Jeor. 1998. Genetic diversity and epidemiology of hantaviruses in Argentina. J. Infect. Dis. 177:529-538[Medline].
20.	Lundkvist, Å., S. Björsten, B. Niklasson, and N. Ahlborg. 1995. Mapping of B-cell determinants in the nucleocapsid protein of Puumala virus: definition of epitopes specific for acute immunoglobulin G recognition in humans. Clin. Diagn. Lab. Immunol. 2:82-86[Abstract].
21.	Lundkvist, Å., A. Fatouros, and B. Niklasson. 1991. Antigenic variation of European haemorrhagic fever with renal syndrome virus strains characterized using bank vole monoclonal antibodies. J. Gen. Virol. 72:2097-2103[Abstract/Free Full Text].
22.	Lundkvist, Å., H. Kallio-Kokko, K. Brus Sjölander, H. Lankinen, B. Niklasson, A. Vaheri, and O. Vapalahti. 1996. Characterization of Puumala virus nucleocapsid protein: identification of B-cell epitopes and domains involved in protective immunity. Virology 216:397-406[Medline].
23.	Lundkvist, Å., and B. Niklasson. 1994. Haemorrhagic fever with renal syndrome and other hantavirus infections. Rev. Med. Virol. 4:177-184.
24.	Lundkvist, Å., O. Vapalahti, A. Plyusnin, K. Brus Sjölander, B. Niklasson, and A. Vaheri. 1996. Characterization of Tula virus antigenic determinants defined by monoclonal antibodies raised against baculovirus-expressed nucleocapsid protein. Virus Res. 45:29-44[Medline].
25.	Medrano, J., E. Aasen, and L. Sharrow. 1990. DNA extraction from nucleated red blood cells. BioTechniques 8:43.
26.	Modi, W. S. 1996. Phylogenetic history of LINE-1 among arvicolid rodents. Mol. Biol. Evol. 13:633-641[Abstract].
27.	Morzunov, S. P., J. E. Rowe, T. G. Ksiazek, C. J. Peters, S. C. St. Jeor, and S. T. Nichol. 1998. Genetic analysis of the diversity and origin of hantaviruses in Peromyscus leucopus mice in North America. J. Virol. 72:57-64[Abstract/Free Full Text].
28.	Myasnikov, Y. A., N. S. Apekina, A. P. Zuevskii, A. V. Khitrin, and A. D. Bernshtein. 1992. The disposition of natural foci of hemorrhagic fever with renal syndrome in different landscape areas of Tyumen Province. Vopr. Virusol. 37:161-165[Medline]. (In Russian.)
28a.	Nemirov, K., O. Vapalahti, Å. Lundkvist, V. Vasilenko, I. Golovljova, A. Plyusnina, J. Niemimaa, J. Laakkonen, H. henttonen, A. Vaheri, A. Plyusnin. 1999. Isolation and characterisation of Dobrava hantavirus carried by the striped field mouse (Apodemus agrarius) in Estonia. J. Gen. Virol. 80:371-379.
29.	Nichol, S. T. Genetic analysis of hantaviruses and their host relationships. In J. F. Saluzz and B. Dodet (ed.), Factors in the emergence and control of rodent-borne viral diseases (hantaviruses and arenaviruses), in press. Elsevier, Paris, France.
30.	Niklasson, B., M. Jonsson, Å. Lundkvist, J. Horling, and E. Tkachenko. 1991. Comparison of European isolates of viruses causing hemorrhagic fever with renal syndrome by a neutralization test. Am. J. Trop. Med. Hyg. 45:660-665.
31.	Page, R. D. M. 1997. Tree map, version 1.0c. University of Glasgow, Glasgow, Scotland.
32.	Plyusnin, A., O. Vapalahti, H. Lankinen, H. Lehväslaiho, N. Apekina, Y. Myasnikov, H. Kallio-Kokko, H. Henttonen, Å. Lundkvist, M. Brummer-Korvenkontio, I. Gavrilovskaya, and A. Vaheri. 1994. Tula virus: a newly detected hantavirus carried by European common voles. J. Virol. 68:7833-7839[Abstract/Free Full Text].
33.	Plyusnin, A., O. Vapalahti, Å. Lundkvist, H. Henttonen, and A. Vaheri. 1996. Newly recognized hantavirus in Siberian lemmings. Lancet 347:1835-1836[Medline].
34.	Plyusnin, A., O. Vapalahti, K. Ulfves, H. Lehvaslaiho, N. Apekina, I. Gavrilovskaya, V. Blinov, and A. Vaheri. 1994. Sequences of wild Puumala virus genes show a correlation of genetic variation with geographic origin of the strains. J. Gen. Virol. 75:405-409[Abstract/Free Full Text].
35.	Plyusnin, A., O. Vapalahti, and A. Vaheri. 1996. Hantaviruses: genome structure, expression and evolution. J. Gen. Virol. 77:2677-2687[Abstract/Free Full Text].
36.	Repenning, C., O. Fejfar, and W.-D. Heinrich. 1990. Arvicolid rodent biochronology of the northern hemisphere, p. 385-418. In International Symposium on Evolution, Phylogeny, and Biostratigraphy of Arvicolids (Rodentia, Mammalia).Pfeil-Verlag, Prague, Czechoslovakia.
37.	Saiki, R., D. Gelfand, S. Stoffel, S. Scharf, R. Higuchi, G. Horn, K. Mullis, and H. Erlich. 1981. Primer-directed enzymatic amplification of DNA with a thermostable DNA polymerase. Science 239:487-491.
38.	Salonen, E.-M., P. Parren, Y. Graus, Å. Lundkvist, P. Fisicaro, O. Vapalahti, H. Kallio-Kokko, A. Vaheri, and D. Burton. 1998. Human recombinant Puumala virus antibodies: cross reaction with other hantaviruses and use in diagnostics. J. Gen. Virol. 79:667-671[Abstract].
39.	Schmaljohn, A. L., D. Li, D. L. Negley, D. S. Bressler, M. J. Turell, G. W. Korch, M. S. Ascher, and C. S. Schmaljohn. 1995. Isolation and initial characterization of a newfound hantavirus from California. Virology 206:963-972[Medline].
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