Robert Koch-Institut, Nordufer 20, 13353 Berlin, Germany1
Institut für Lebensmittel, Arzneimittel und Tierseuchen, Invalidenstr. 60, 10557 Berlin, Germany2
Institut für Veterinär-Pathologie der Freien Universität Berlin, Straße 518, Nr. 15, 14163 Berlin, Germany3
Zoologischer Garten Berlin AG, Hardenbergplatz 8, 10787 Berlin, Germany4
Author for correspondence: B. Ehlers. Fax +49 1888 754 2598. e-mail EhlersB{at}RKI.DE
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Abstract |
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Introduction |
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In the present study, we identified ElHV-1 in affected organ material from Kiba by ultrastructural analysis and partially characterized its genome. Genetic analysis was achieved by using (i) a pan-herpes consensus PCR to get access to the DNA polymerase (DPOL) gene and (ii) a PCR-based genome walking technique to amplify and sequence the complete DPOL gene as well as the complete glycoprotein B (gB) gene. Our goals were to elucidate firmly the evolutionary relatedness of ElHV-1 to other herpesviruses, to develop a sensitive nucleic acid-based detection method for herd control in zoological gardens and to identify a glycoprotein gene that can be used for the development of an ELISA and can serve as a basis for a vaccination approach.
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Methods |
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Sample collection and preparation of DNA.
Organ and serum samples were collected post-mortem from the male elephant Kiba, which died from endothelial disease in the zoological garden of Berlin in 1998. Serum samples from his offspring Plai Kiri and other members of the herd were collected in 2000. Total tissue DNA was prepared with the QIAamp DNA tissue kit. Serum was processed with the QIAamp DNA blood kit (Qiagen).
Pan-herpes consensus PCR and genome walking.
Pan-herpes consensus PCR was performed as described previously (Ehlers et al., 1999a , b
). Genome walking was used to extend the initial 178 bp sequence obtained by pan-herpes consensus PCR and was performed by Genexpress GmbH (Berlin), as described previously (Ulrich et al., 1999
). Sequence analyses were done by Agowa GmbH (Berlin).
ElHV-specific long-range PCR.
The primer combinations U4 (5' GGGTCTATGTTCACGTCCTC 3') plus D2 (5' CTGTCGCTGCACATGCATCG 3') and U4 plus D1 (5' CGTAATTAGCAACTCTCTCG 3') were used by Agowa GmbH for amplification of 6839 and 6410 bp fragments of ElHV-1 DNA with the Expand High Fidelity PCR kit (Roche AG).
ElHV-specific nested PCR.
PCR was carried out with 100 ng tissue DNA or 1 µl serum processed with the QIAamp DNA blood kit to an equal volume of eluate. In the second round of nested PCR, 1 µl of the first-round PCR was used as template. Reaction mixtures (50 µl) were set up with the HotStarTaq Mastermix kit (Qiagen) according to the manufacturers instructions. For thermal cycling, Perkin-Elmer 2400 thermocyclers and 0·2 ml thin-wall tube strips were used. The primer combination El_DPOL_2s (sense; 5' ACGCAGCACTTGTTTACATTAGG 3') plus El_DPOL_2as (anti-sense; 5' AGAACTGGGATCTGCTTGTATGA 3') was used in the first-round PCR (428 bp) and the primer combination El_DPOL_3s (sense; 5' CTGGAGGGTCTACGGTCCAAATT 3') plus El_DPOL_3as (antisense; 5' CTGCTTGTATGAAACGGAGTGTT 3') was used in the second round (316 bp). In the first-round PCR, the reaction mixtures were kept at 95 °C for 15 min and then cycled 40 times with 1 min denaturation at 94 °C, 1 min annealing at 63 °C and 1 min strand extension at 72 °C, followed by a final extension step at 72 °C for 5 min. In the second-round PCR, conditions were identical except that the annealing temperature was 65 °C.
Nucleotide and protein sequence analysis.
Multiple sequence alignments were performed and protein pair distances calculated with the clustalW module of MacVector (version 6.01, Oxford Molecular Group). For phylogenetic analysis, gaps or insertions unique to a particular species were removed from the multiple sequence alignments and the remaining conserved regions were concatenated for each individual protein (McGeoch et al., 1995 ). Trees were then constructed with the PHYLIP package using the programs Protdist (Dayhoff PAM matrix) and Neighbor or, alternatively, the program Protpars with randomized input of sequences. The trees were evaluated statistically by bootstrap analysis (1000-fold resampling) by using the programs Seqboot and Consense (Felsenstein, 1985
, 1993
).
The following herpesvirus gB and DPOL genes were included in comparative analyses of amino acid and nucleotide sequences. Alphaherpesvirinae: AtHV1 (ateline herpesvirus-1) (gB, accession no. M95785); BoHV1 (bovine herpesvirus-1) (gB, accession no. M21474; DPOL, accession no. Z78205); BoHV2 (gB, accession no. M21628; DPOL, accession no. AF181249); CeHV1 (cercopithecine herpesvirus-1) (gB, accession no. U14664); EHV1 (equine herpesvirus-1) (gB and DPOL, accession no. M86664); EHV4 (gB and DPOL, accession no. AF030027); FeHV1 (feline herpesvirus-1) (gB, accession no. S49775; DPOL, accession no. AJ224971); GaHV1 (gallid herpesvirus-1 or infectious laryngotracheitis virus) (gB, accession no. X56093); GaHV2 (Mareks disease virus) (gB, accession no. D13713; DPOL, accession no. L40431); HSV1 (herpes simplex virus type 1 or human herpesvirus-1) (gB and DPOL, accession no. X04771); HSV2 (human herpesvirus-2) (gB and DPOL, accession no. Z86099); HVP-2 (herpesvirus papio 2) (gB, accession no. U14662); MaHV1 (macropodid herpesvirus-1 or kangaroo herpesvirus) (gB, accession no. AF061754); PRV (pseudorabies virus or suid herpesvirus-1) (gB, accession no. M17321; DPOL, accession no. L24487); VZV (varicella-zoster virus or human herpesvirus-3) (gB and DPOL, accession no. X04370); PhHV1 (phocid herpesvirus-1) (gB, accession no. Z68147) and SaHV1 (saimirine herpesvirus 1) (gB, accession no. M95786). Betaherpesvirinae: CaHV2 (caviid herpesvirus 2 or guinea pig cytomegalovirus) (gB and DPOL, accession no. L25706); CeHV8 (rhesus monkey cytomegalovirus) (gB, accession no. U76749; DPOL, accession no. AF033184); HCMV (human cytomegalovirus or human herpesvirus-5) (gB and DPOL, accession no. X17403); HHV6 (human herpesvirus-6) (gB and DPOL, accession no. X83413); HHV7 (gB and DPOL, accession no. U43400); MCMV (murine cytomegalovirus or murine herpesvirus-1) (gB and DPOL, accession no. U68299); MuHV2 (murine herpesvirus-2 or rat cytomegalovirus) (gB and DPOL, accession no. U50550); TuHV1 (Tupaia herpesvirus-1) (gB, accession no. AF084543; DPOL, accession no. AF074327). Gammaherpesvirinae: AlHV1 (alcelaphine herpesvirus-1) (gB and DPOL, accession no. AF005370); BoHV4 (gB, accession no. Z15044; DPOL, AF271211); EBV (EpsteinBarr virus or HHV4) (gB and DPOL, accession no. X00784); EHV2 (gB and DPOL, accession no. U20824); EHV5 (gB, accession no. AF050671); HHV8 (gB and DPOL, accession no. U75698); HVS (herpesvirus saimiri or SaHV2) (gB and DPOL, accession no. X64346); HVA (herpesvirus ateles or AtHV2) (gB and DPOL, accession no. AF083424); MHV68 (murine gammaherpesvirus-68) (gB and DPOL, accession no. U97553); PLHV1 (porcine lymphotropic herpesvirus-1) (DPOL, accession no. AF191042); PLHV2 (DPOL, accession no. AF191043); RRV (rhesus monkey rhadinovirus) (gB and DPOL, accession no. AF029302).
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Results |
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Analysis of the gB gene
The ElHV-1 gB deduced from the gB ORF has a length of 845 amino acids. It shows the typical features of a membrane-bound glycoprotein. The N terminus contains a hydrophobic stretch (aa 2438) that may constitute a signal sequence and, in the C-terminal part, there are other hydrophobic stretches (aa 700750) that may function as transmembrane sequences (Fig. 2c). Seventeen cysteine residues are present, nine of which show positional conservation in the gBs of all other herpesviruses analysed. Furthermore, 11 potential N-glycosylation motifs and a putative endoproteolytic cleavage site (ArgArgLysArg433) (Spaete et al., 1990
; Wellington et al., 1996
) were found in ElHV-1. The sequences CYSRP (aa 552555), GQLG (aa 573576) and NPFG (aa 726729) in ElHV-1 gB are well conserved amongst other herpesvirus gB genes.
In amino acid sequence comparisons, the ElHV-1 gB was most closely related to those of HHV6 and HHV7; however, the identity was only 32%. Other betaherpesviruses revealed 2830% identity and alpha- and gammaherpesviruses respectively revealed 2122% and 2526% identity. In phylogenetic analysis with the neighbour-joining method (programs Protdist and Neighbor), ElHV-1 gB did not cluster with any of the herpesvirus subfamilies but instead formed a separate branch between the Betaherpesvirinae and the Gammaherpesvirinae (Fig. 3a). Also, in parsimony analysis (program Protpars), ElHV-1 gB branched close to the central point that segregates the three virus subfamilies (not shown).
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Two partial ORFs were identified, one located upstream of the gB gene and the other located downstream of the DPOL gene in the reverse orientation (Fig. 2b). The encoded proteins are also most closely related to the corresponding positional homologues of betaherpesviruses (ORFs 40 and 37 of HHV6; ORFs 56 and 53 of HCMV).
These genetic data show that a set of genes exists in ElHV-1 that are identical in arrangement with the respective gene blocks of the betaherpesviruses. However, the amino acid identity does not exceed 40%, indicating a comparatively distant relationship. This is supported by the phylogenetic trees (Fig. 3a, b
).
ElHV-specific nested PCR
We set up an ElHV-specific nested PCR that is based on the DPOL gene and amplifies a 316 bp fragment in the second-round PCR. With this PCR system, heart and liver specimens and a serum sample taken from Kiba after his death in 1998 were analysed. Serum samples taken in 2000 from his offspring Plai Kiri, Plai Kiris mother Pang-Pha and the herd members Svea, Ayesha, Iyoti and Drumbo were also analysed. In the first and the second round of the nested PCR, the organ specimens and the serum from Kiba were strongly ElHV-1 positive. The serum samples from Plai Kiri and other herd members were negative (Fig. 4).
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Discussion |
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For genetic characterization of ElHV-1, the gB and DPOL genes as well as flanking genes were analysed. Although only moderate identity values (<40%) were found in pairwise comparisons of gB and DPOL with those of other herpesviruses, the identification of conserved and functional sites in both gB and DPOL (Fig. 2c) unequivocally validated their identification. On the basis of the sequences of both genes, ElHV-1 was most closely related to the betaherpesviruses. The partial ORFs identified in the flanking regions were also found to be positional homologues of betaherpesvirus genes. Therefore, the identified gene block is betaherpesvirus-like. A low G+C content (40 mol%) was found, but no significant deviation from the expected CpG dinucleotide frequency was apparent (Honess et al., 1989
). In this respect, ElHV-1 is also more similar to the betaherpesviruses than to the other two subfamilies. However, in phylogenetic analysis of gB and DPOL, ElHV-1 appeared to be distantly related to all three herpesvirus subfamilies, with a long separate branch that was slightly closer to the Betaherpesvirinae than to the Gammaherpesvirinae (Fig. 3a
, b
). Therefore, ElHV-1 might be classified as a member of the Betaherpesvirinae, but it would obviously constitute a new genus. Alternatively, ElHV-1 might be a member of a new herpesvirus subfamily; this can only be clarified by analysis of the complete ElHV-1 genome.
The sequence of the complete DPOL gene determined from the German ElHV-1 isolate in this study was compared with the 0·1 kbp DPOL sequences of ElHV-1 amplified from Asian elephants in North America (Richman et al., 1999 ). One silent base exchange was found (not shown). A similar observation was made in a comparison of terminase gene sequences (Burkhardt et al., 1999
). This indicates that the German ElHV-1 isolate and the North American isolates have nearly identical genomes. In phylogenetic analysis with the neighbour-joining method, the American 0·1 kbp DPOL sequence also clustered close to the centre of the herpesvirus tree, but slightly closer to the Alphaherpesvirinae (Richman et al., 1999
). This result is not in complete accord with our results, but this can be attributed to the shortness of the sequence. Further genetic characterization of the American isolates is needed for a more accurate comparison.
A sensitive nested-PCR assay was developed for the detection of ElHV-1. This assay can be used by zoological gardens to control suspected cases of endothelial inclusion body disease in their elephant herds, as demonstrated by the post-mortem analysis of Kiba and the analysis of serum from his offspring, Plai Kiri, and other Asian elephants at the Berlin zoo (Fig. 4). Detection of viraemia by PCR at an early stage of the disease could verify the clinical diagnosis of endothelial inclusion body disease and allow a timely attempt at treatment with an anti-herpesvirus drug, as was reported by Schmitt & Hardy (1998)
, who successfully used famciclovir in the treatment of a herpesvirus-infected, clinically ill Asian elephant. However, routine PCR analysis of blood of healthy elephants is probably not feasible, because detection of ElHV-1 in the blood might simply indicate latent virus in peripheral blood leukocytes (PBL) and not an acute disease process. Since the ability to establish a latent state is a general feature of herpesviruses of all three subfamilies (Stanberry, 1986
; Stevens, 1989
), this must also be assumed for ElHV-1. The nested-PCR assay presented in this study will help to identify such sites of ElHV latency. Preliminary analyses of PBL samples from the herd in Berlin (data not shown) revealed no evidence of ElHV-1 latency in PBL. However, this issue requires additional testing of Asian elephants from other locations.
Finally, the identification of the gB gene offers the opportunity to develop an ElHV-specific ELISA and other antibody-based detection methods that can aid in the diagnosis of the disease and detection of carrier animals. Furthermore, vaccination strategies by DNA immunization with a gB-recombinant expression vector or by infection with gB-expressing recombinant viruses can be envisaged, providing a potential tool for the protection of the endangered Asian elephant.
Note added in proof. Kiri, the offspring of Kiba, died on 28 December 2000, after an overnight peracute course of illness of only approximately 6 h. Pathological inspection showed multiple organ alterations very similar to those of Kiba. All organs analysed by nested PCR were strongly ElHV-1-positive, including liver, heart, kidney, intestine and blood. In addition, herpesvirus-like particles were found by electron microscopy.
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Acknowledgments |
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Footnotes |
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References |
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Received 14 September 2000;
accepted 14 November 2000.
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