Comparison of the Complete DNA Sequences of Human Herpesvirus 6 Variants A and B

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Journal of Virology, October 1999, p. 8053-8063, Vol. 73, No. 10
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Comparison of the Complete DNA Sequences of Human Herpesvirus 6 Variants A and B

Yuji Isegawa,^* Tetsu Mukai, Kazushi Nakano, Miwa Kagawa, Jiguo Chen, Yasuko Mori, Tomimasa Sunagawa, Kazunobu Kawanishi, Junji Sashihara, Atsuko Hata, Ping Zou, Haruhiko Kosuge, and Koichi Yamanishi

Department of Microbiology, Osaka University Medical School C1, 2-2 Yamada-Oka Suita, Osaka 565-0871, Japan

Received 19 April 1999/Accepted 14 June 1999

	ABSTRACT

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Human herpesvirus 6 (HHV-6), which belongs to the betaherpesvirus subfamily and infects mainly T cells in vitro, causes acuteand latent infections. Two variants of HHV-6 have been distinguishedon the basis of differences in several properties. We have determinedthe complete DNA sequence of HHV-6 variant B (HHV-6B) strain HST,the causative agent of exanthem subitum, and compared the sequencewith that of variant A strain U1102. A total of 115 potentialopen reading frames (ORFs) were identified within the 161,573-bpcontiguous sequence of the entire HHV-6 genome, including somegenes with remarkable differences in amino acid identity. Allgenes with <70% identity between the two variants were found tocontain deleted regions when ORFs that could not be expressedwere excluded from the comparison. Except in the case of U47,these differences were found in immediate-early/regulatory genes,DR2, DR7, U86/90, U89/90, and U95, which may represent characteristicdifferences of variants A and B. Also, we have successfully typed14 different strains belonging to variant A or B by PCR usingvariant-specific primers; the results suggest that the remarkabledifferences observed were conserved evolutionarily as variant-specificdivergence.

	INTRODUCTION

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Human herpesvirus 6 (HHV-6) was first isolated in 1986 from the peripheral blood of patients with lymphoproliferative disorders(53). By comparison with other human herpesviruses, molecularand immunological analyses revealed its distinct nature (22).The virus replicates predominantly in CD4⁺ lymphocytes (33, 60) and may establish latent infection incells of the monocyte/macrophage lineage (23). Infection withthis virus results in exanthem subitum (ES), a common illnessof infancy (74), but has not yet been clearly linked to anydisease in adults. Two variants of HHV-6 have been identifiedon the basis of differences in epidemiology, in vitro growth properties,reactivity with monoclonal antibodies, restriction endonucleasemapping, and nucleotide sequence (1, 2, 8, 15, 55,72, 73), leading to adoption of the nomenclature HHV-6A (variantA) and HHV-6B (variant B). HHV-6A has not yet been clearly linkedto any disease, and HHV-6B is the causative agent of ES (3).Gompels and coworkers (16) have determined the complete DNAsequence of HHV-6A strain U1102. In the present report, to examinewhich gene(s) could be related to pathogenicity and other viralproperties, we present the complete DNA sequence of HHV-6 strainHST, which belongs to variant B, and compare the sequence withthat of HHV-6A. We also report that some of the HHV-6 genes showremarkable differences in deduced amino acid sequence identitycompared with variant A. Such differences could represent characteristic,or possibly pathogenic, differences between the twovariants.

	MATERIALS AND METHODS

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Cells and viruses. Umbilical cord blood mononuclear cells (CBMCs) were separated on a Ficoll-Conray gradient, cultured in RPMI 1640 medium containing10% fetal calf serum, and stimulated with phytohemagglutinin (5µg/ml) for 2 or 3 days. HHV-6 strain HST, which was isolated froma patient with ES and belongs to the variant B group, was propagatedin fresh human peripheral mononuclear cells (74). To preparevirus stocks, virus was propagated in stimulated CBMCs. When morethan 80% of the cells showed cytopathic effects, the culture ofinfected cells was frozen and thawed twice; after centrifugationat 1,500 × g for 10 min, the supernatant fraction was stored at $-$ 80°C as a cell-free virus stock. To infect cells with virus,stimulated CBMCs (10⁷ cells) were washed twice with phosphate-buffered saline, suspendedin 1 ml of virus solution with 10⁷ 50% tissue culture infective doses per ml, and spun at 1,500× g for 40 min at 37°C for adsorption. To prepare the viral DNA,the infected cells were cultured for 2 or 3 days in RPMI 1640medium supplemented with 10% fetal calf serum and harvested whenapproximately 50% of the cells showed cytopathic effects. Foranalysis of independently isolated viruses by PCR, CBMCs infectedwith the viruses were used. The following viruses were kindlysupplied by other researchers: strain Z29 by C. Lopez (32),strains GS and DA by D. V. Ablashi (1), strain U1102 by R.Honess (11), and strain St. W. by G. Enders (12). Other HHV-6strains (MNM1, MNM2, TMK1, TMK2, NKT2, OKC1, OKC3, and MCZ2) wereisolated in our laboratory from patients with ES. All strainswere confirmed as HHV-6 by using specific monoclonal antibodiesto HHV-6 (data not shown). To test the specificities of the primersused for conducting virus strain typing, herpes simplex virustype 1 (HSV-1; strain F), HSV-2 (strain G), varicella-zoster virus(strain Oka), human cytomegalovirus (HCMV; strain AD169), Epstein-Barrvirus (strain B95-8), and HHV-7 (strain KHR) were used forPCR.

Preparation and purification of HHV-6 DNA. To determine the DNA sequence of the entire HHV-6 HST genome, viral genomic DNA was purified as described elsewhere (35,43). To amplify HHV-6 genome DNA by PCR, DNA from HHV-6-infectedCBMCs (10⁶ cells) 2 days after infection was extracted in 0.5 ml of lysisbuffer (0.45% Nonidet P-40, 0.45% Tween, 10 mM Tris-HCl [pH 8.3],50 mM KCl, 3 mM MgCl₂, 10 µg of protease K per ml) at 65°C overnightand at 98°C for 10 min to denature the proteinaseK.

PCR. For assembling the various DNA sequences into the complete genome DNA sequence, the junction regions of nonoverlapping sequences,except the origin of DNA binding (Ori) region, the 3' end of theunique region, and the concatemer junction region, were amplifiedby PCR using genomic viral DNA prepared as described above withcorresponding oligonucleotide primers, which were synthesizedbased on the previously determined HHV-6 sequence at the fragmenttermini. PCR was carried out with approximately 10 ng of the viralDNA template as follows: 25 cycles of denaturation (95°C for 1min), annealing (55°C for 1 min), and extension (72°C for 2 min),using a PCR Thermal Cycler TP480 (Takara Shuzo, Kyoto, Japan).For the Ori region and the right-hand end of the unique region,amplified DNA fragments were obtained from 10 ng of purified strainHST DNA by shuttle PCR as described below, using LA Taq (TakaraShuzo), an appended buffer, 200 µM each deoxynucleoside triphosphate,and two pairs of PCR primers, 06-3end (5'-AAGACACCATACTCGGAAGAATCATGTTACGACGTT)-22-5end(5'-TTGGCCTGAGACCTTACAACGGAGACGCCCGTGATC) and 07-5end (5'-GAGATAGAGTCGGCCTTGGAACACGTCGTGGCAGAAC)-45-3end(5'-GATAAAAAAGTAATTCGTTCATATGAGTAGTCGGAT), respectively. In thecase of the concatemer junction region, the DNA fragment was obtainedfrom extracted viral DNA by shuttle PCR as described below, usingprimers 5Ter-JuncC.LA (5'-CAGGGCGTGGCTGACACGCGCCGGCAGCGGCAT) and3Ter-JuncF.LA (5'-ACGACGCCAAGGGAAGCCTCTGGCGCAATCTAT). The PCRproduct was then cloned into vector pCR2.1 (Invitrogen, San Diego,Calif.). Shuttle PCR conditions were as follows: incubation at98°C for 3 min for hot start, 30 cycles of 98°C for 30 s, and68°C for 10 min, with a final extension at 72°C for 10min.

DNA sequencing and sequence analysis. Purified viral genomic DNA was digested with restriction enzymes PstI, BamHI, HindIII, or KpnI (Takara Shuzo). The resultantfragments were cloned into the corresponding restriction enzymesites of pUC19. To make deletion libraries, pUC19 clones carryingPstI-DNA fragments (designated pSTY clones) and the other restrictionfragments (Fig. 1) were subjected to unidirectional progressivedeletions, except for pSTY57, which contained an insert of approximately200 bp. This procedure was carried out with a deletion kit forkilo-sequencing (Takara Shuzo), and the DNAs were subsequentlytransformed into Escherichia coli to obtain the correspondingdeletion mutants. These inserts, as well as the normal PCR productsdescribed above, were sequenced as described by Isegawa et al.(20). Their corresponding sequences were confirmed by usingthe opposite unidirectional progressive deletions of the pSTYclones, the cassette-ligation-mediated PCR method, or direct sequencingof PCR products amplified from DNA (20). The resultant shuttlePCR products mentioned above were directly sequenced by cassette-ligation-mediatedPCR (20) using a Li-Cor (Lincoln, Neb.) 4000L DNA sequencer.The nucleotide sequence of the entire HHV-6 genome thus obtainedwas analyzed to identify potential open reading frames (ORFs),using the software packages MacDNASIS version 3.7 (Hitachi SoftEngineering Co., Ltd., Yokohama, Japan) and ALIGN (Genome InformationResearch Center, Osaka University). Sequence comparisons werecarried out using the sequences of HHV-6A (strain U1102) (16),HHV-6B (strain Z29) (9, 26, 27, 48), and HHV-7 (strainJI) (44).

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FIG. 1. Restriction fragments used for the sequencing of HHV-6 strain HST. The HHV-6 genome is represented diagrammatically, together with the positions of BamHI, HindIII, KpnI, and PstI sites. Various plasmid-cloned restriction fragments are prefixed with Ba, H, Kp, or pSTY (indicating their terminal restriction sites). Sequenced restriction fragments are indicated by shading.

Nucleotide sequence accession number. The complete sequence of HHV-6 strain HST has been deposited in the GenBank, EMBL, and DDBJ Data Libraries under accessionno. AB021506.

	RESULTS

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Assembling the contiguous HHV-6B sequence. The HHV-6 genome was sequenced by using the PstI, BamHI, HindIII, and KpnI deletion libraries described above. The fragmentsused for the project are shown in Fig. 1. The resultant PstI-DNAfragments of 15.3, 13.1, 9.7, 6.6, 6.5, 5.5, 5.3, 5.3, 5.2, 4.8,4.6, 4.5, 4.4, 4.4, 4.1, 3.8, 4.0, 2.5, 2.7, 2.1, 1.7, 1.7, 1.5,1.5, 1.5, 1.4, 1.2, 1.2, 1.1, 1.0, 1.0, 0.8, 0.7, and 0.2 kb werecloned into pUC19 and designated pSTY01, -02, -03, -05, -06, -07,-08, -09, -10, -13, -15, -16, -22, -23, -24, -27, -28, -29, -32,-34, -36, -37, -41, -42, -43, -45, -46, -47, -48, -49, -50, -52,-56, and -57, respectively. These pSTY clones covered about 85%of the HHV-6 genome. Junctions between nonoverlapping restrictionfragments were determined by directly sequencing PCR fragmentsspanning the junction regions (see Materials and Methods). Thesequences of the terminal direct repeat (DR) elements were derivedby compiling partial sequences of DR_L and DR_R to generate thecomplete DR sequences. The positions of the left and right genometermini were determined by sequencing PCR fragments that had beenproduced with 5'- and 3'-terminal concatemer junction primers(see Materials and Methods). As shown in Fig. 2, the HHV-6 genomewas composed of the DRs at the left and right ends of the genome(DR_L and DR_R) and the unique region (UR; containing the repeatregions [R1, R2, and R3] and Ori), for a total of 161,573 bp,including 8,231 bp in the DRs (DR_L, nucleotide positions 1 to8231; DR_R, nucleotide positions 153,333 to 161573) and 145,101bp in the UR (nucleotide positions 8232 to 153332). The genomelength of the HST strain was 2,244 bp larger than that of theU1102 strain (144 and 1,966 bp larger at DR and UR, respectively).The overall GC content of the HST strain was 43%, the same asthat of the U1102 strain. When the nucleotide sequence was comparedwith that of the U1102 strain, marked differences were observedonly at specific regions of the DR and at the junction betweenthe UR and DR. Higher similarity was observed in the UR. The nucleotidesequence variation of these regions is attributable differencesbetween strains rather than differences between variants (43).

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FIG. 2. Predicted ORF organization of HHV-6 strain HST. Repeat regions (DR_L, DR_R, R1, R2, and R3) are boxed; telomeric repeat regions (T1 and T2) are denoted by striped bars; UR is indicated by a solid line. Protein coding regions are indicated as open arrows and are numbered DR1, DR2, DR3, DR6, DR7, DR8, DRHN1, and DRHN2 within the direct repeats and HN1, HN2, HN3, and U1 to U100 (excluding U78, U88, U92, U93, and U96) within the UR. The Ori is indicated by an asterisk. These regions are further described in Table 1 and in the text. The US22 gene family is shaded. Abbreviations not given in text: GCR, G-protein-coupled receptor; Ig, Ig immunoglobulin superfamily; RR, large subunit of ribonucleotide reductase; mCP, minor capsid protein; CA, capsid assembly protein; Teg, tegument protein; Pol, DNA polymerase; tp, transport protein; mDBP, major single-stranded DNA binding protein; TA, conserved herpesvirus transactivator; dUT, dUTPase; Pts, protease/assembly protein; pp65/71, phosphoprotein 65/71K; MCP, major capsid protein; PT, phosphotransferase; Exo, exonuclease; OBP, origin binding protein; Hel, helicase; UDG, uracil-DNA glycosylase; Che, chemokine; AAV rep1, adeno-associated virus replication protein homolog.

Identification of HHV-6B ORFs. The contiguous 161,573-bp sequence of the entire HHV-6 genome was analyzed to identify potential ORFs, using DNASIS version3.7 (Hitachi Soft Engineering). Potential genes in the HHV-6 strainHST genome were selected by the following criteria: (i) ORFs largerthan 300 nucleotides with initiating methionine codons (ATG) weregenerally considered to be genes encoding proteins; and (ii) ORFssmaller than 300 nucleotides but larger than 80 nucleotides wereconsidered to be genes if their deduced amino acid sequences showedsignificant homology to those of U1102 and other herpesvirusesor cellular proteins. The ORFs and homologous regions thus identifiedare illustrated in Fig. 2 and listed in Table 1. Within the DR,there are several ORFs (LT1, DR1, DR2, DR3, DR6, DR7, DR8, DRHN1,and DRHN2), and numerous ORFs are present within the UR. In general,the degrees of identity between corresponding ORFs were very highbetween variants A and B (Table 1). However, variant-specificORFs were observed in the genome of each strain: HN1, HN2, HN3,DRHN1, and DRHN2 in the HST strain and U78, U88, U92, U93, U96,DR4, and DR5 in the U1102 strain. HN1 and HN3 turned out to beexons of the U89-IE1 (immediate-early 1) and spliced glycoproteingp82/105 genes, respectively, when their cDNAs were analyzed.The functions of these variant-specific ORFs are not clear. Itis possible that some ORFs may not encode functional proteinsat all. However, it is conceivable that the others are associatedwith biological and pathogenic differences between variants Aand B.

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TABLE 1. ORF identity between HST and U1102 strains of HHV-6

Comparisons of ORFs between HHV-6 variants. Sequence alignments of ORFs in the UR between the HST and U1102 strains indicated that the amino acid identity between theseviruses was about 94% on average, except for the variant-specificORFs. Putative functions of the various HHV-6 genes implicatedby their corresponding homologs are listed in Table 1, whichshows that 67 of the 103 ORFs compared exhibited >90% identitybetween these strains. As shown in Table 1, ORFs with 80 to 90%identity were DR1, DR3, DR6, U8, U11, U12, U14, U15, U18, U21,U23, U65, U71, U80, and U83. Of these, U8 and U18 were IE/regulatorygenes, U80 was a replication gene, U12, U21, and U23 encoded glycoproteins,U11 encoded a viral protein, and U83 encoded a chemokine (76).ORFs with 70 to 80% identity were U54, U79, U91, U97, U98, U99,and U100. U79 was a replication gene, U97, U98, U99, and U100encoded glycoproteins, and U54 was a viral protein gene. ORFswith <70% identity were LT1, DR2, DR7, DR8, LJ1, RJ1, U1, U47,U86, U89, U90, and U95. It is possible that high divergence inamino acid sequence leads to biological and pathogenic differencesbetween variants A and B. Some of these 12 divergent genes couldbe directly involved in such functional differences. The ORFswith different starting or termination sites were classified ashaving different sizes if the difference was more than five deducedamino acid residues. The ORFs with different starting sites wereDR2, DR7, DR8, LJ1, U1, U2, U3, U7, U8, U21, U23, U47, U55, U83,U98, and U100. The ORFs with different termination sites wereDR7, DR8, LJ1, U1, U10, U20, and U47. The ORFs containing insertionswere DR2, DR3, DR7, U11, U47, U86, U89, and U95. Finally, in thecase of the chemokine receptor (U12) and gp82/105 (U97, HN3, U98,U99, and U100), the differences were due to differentialsplicing.

(i) IE/regulatory genes. IE proteins control the temporal cascade of gene expression and are a second line for determining the cellular specificityof infection. Based on in vitro chloramphenicol acetyltransferaseor luciferase assays, at least eight genes that might serve astranscriptional activators have been defined: DR7, U3, U16/U17,U18/U19, U27, U86, U89, and U94 (13, 34, 42, 46, 66,67, 75). There are multiple US22 genes in HCMV, HHV-6, andHHV-7 (5), and this feature appears to be a characteristicof the betaherpesvirus subgroup (7, 16). The translationproducts of these genes in strain HST differed greatly in length(89 to 1,197 amino acid residues), but they each contained atleast one of four US22 amino acid sequence motifs (7, 16).This US22 gene family of HCMV is transcribed with IE kineticsand possesses transactivating functions (57). Strain HST contained11 ORFs of the US22 gene family: DR1, DR2, DR6, DR7, U2, U3, U7,U8, U16, U25, and U95 (Table 1 and Fig. 2). cDNA analysis showedthat HN1 and U90 corresponded to exons of both the IE1 and IE2genes, which also contained U89 and U86, respectively (18).Amino acid sequence comparisons also suggested that other regions,including U42 and U54, could be involved in transcriptional activation.U42 is a member of the only family of genes involved in transactivationthat is conserved among all of the herpesviruses. An HCMV homolog,UL69, has been shown to transactivate gene expression in vitro(71), but studies of the HSV-1 homolog showed that it also hasroles in transcriptional termination and in snRNP distribution(37, 51). U54 has similarity to the duplicated genes UL82and UL83 of HCMV, and UL82 has been shown to be a transcriptionalactivator and a component of the tegument (29). It is noteworthythat the adeno-associated virus 2 rep gene homolog identifiedin HHV-6, capable of specifying transregulatory and adeno-associatedvirus 2 DNA replication functions, was absent in other herpesviruses(67, 68). Among the IE/regulatory genes (DR1, DR2, DR6, DR7,U2, U3, U7, U8, U16, U17, U18, U19, U25, U27, U42, U54, U86/U90,U89/U90, U94, and U95), amino acid sequence comparisons revealedthe following amino acid sequence identities between strains HSTand U1102: U2, U3, U7, U16, U17, U19, U25, U27, U42, and U94,>90%; DR1, DR6, U8, and U18, 80 to 90%; U54, 79.5%; and DR2, DR7,U86, U89, U90, and U95, <70%.

(ii) Replication genes. Each herpesvirus that has been sequenced contains a set of conserved replication genes that are essential for viral DNA replicationduring productive infection. The core replication genes in HHV-6were those encoding DNA polymerase (U38), DNA polymerase processivityfactor (U27), a major DNA binding protein (a single-stranded DNAbinding protein; U41), and components of the heterotrimeric helicase/primasecomplex (U43, U74, and U77). Other genes necessary for DNA replicationwere specific to herpesvirus subgroups and/or particular viruses.The alphaherpesvirus origin binding protein homolog encoded byHHV-6 (U73) presumably is also functionally analogous (17, 25).The UL84, UL112, and UL113 genes of HCMV likely encode proteinsessential for replication functions, such as those enhancing theexpression of the replication genes (21). HHV-6 encoded U55,U79, and U80, which were homologous to UL84, UL112, and UL113,respectively (16). Comparison of the deduced amino acid sequencesof the replication genes (U27, U38, U41, U43, U55, U73, U74, U77,U79, and U80) and revealed that U27, U38, U41, U43, U55, U73,U74, and U77 showed >90% identity between strains HST and U1102and that U79 and U80 showed 77.4 and 81.0% identities, respectively.cDNA analysis showed that U80 was an exon of U79, and five differentcDNAs were expressed from this region in infected cells, due toalternative splicing (65). All replication genes except U79and U80 were highly conserved between the two variants. Theseresults suggest that replication genes may not contribute to thebiological differences between these twovariants.

(iii) Nucleotide metabolism and DNA repair. We identified HHV-6 homologs of herpesvirus gene products that are involved indirectly in DNA replication by acting as nucleotidesubstrates or through DNA repair. These gene products includedribonucleotide reductase (U28), dUTPase (U45), phosphotransferase(U69), alkaline exonuclease (U70), and uracil-DNA glycosylase(U81). The ribonucleotide reductase homolog of HHV-6 was encodedby a single ORF specifying a single protein (7, 15, 44),as is the case in the other betaherpesviruses (HHV-7 and HCMV),while the ribonucleotide reductase homolog of alphaherpesvirus,gammaherpesvirus, and cells is formed with subunits. HHV-6 wassensitive to ganciclovir (6, 41), though we do not know whichgene(s) is associated with the phosphorylation of ganciclovir.The phosphotransferase gene product of HCMV (UL97), which is ahomolog of HHV-6 U69, can phosphorylate nucleotides and the antiviralnucleoside analogue ganciclovir (28, 58). The HHV-6 dUTPaseand uracil-DNA glycosylase homologs presumably specify enzymaticactivities involved in the excision of uridine residues from DNA,like the U81 gene product, which possesses uracil-DNA glycosylaseactivity when expressed in E. coli (54). Among HHV-6 ORFs, allof the genes involving nucleotide metabolism and DNA repair (U28,U45, U69, U70, and U81) were strictly conserved, exhibiting morethan 94% identity between strains HST and U1102. These resultssuggest that nucleotide metabolism and DNA replication genes maynot be involved in the functional divergence between variantsA andB.

(iv) Glycoproteins. In all sequenced herpesviruses, there are conserved glycoprotein genes encoding glycoprotein B (gB), gH, gM, and gL, all ofwhich were also conserved in HHV-6 (U39, U48, U72, and U82, respectively).gB and gH are structurally highly conserved between herpesviruses,are membrane bound, and appear to play roles in virus-cell fusionand cellular spread of virus infection. Both gB and gH of HHV-7are encoded by late genes (56), whereas gB and gH of HHV-6 areencoded by IE and early-late genes, respectively (19, 39).However, the actual translation of the gB gene of HHV-6B occursat the late phase (63). These results suggest that the gB geneof HHV-6 is regulated posttranscriptionally. gL physically associateswith the gH precursor protein and may be required for gH transportand/or processing (30, 31). gM is fairly conserved betweenherpesviruses and was shown to be a component of the virus particlein HSV-1 and equine herpesvirus type 1 (4, 52).

HHV-6 contained two genes (U12 and U51) encoding G-protein-coupled receptor homologs. U12 functionally encodes a calcium-mobilizingreceptor for the $beta$ -chemokines RANTES, MIP-1 $alpha$ and -1 $beta$ , and MCP-1but not for the $alpha$ -chemokine interleukin-8 (19). HHV-6 U51 wasa positional and structural homolog of the HHV-7 and HCMV UL78,showing relatively high sequence similarity to the G-protein-coupledreceptor of herpesvirus saimiri (15, 45). This similaritycould be an indication that they were derived from the same genewithin a progenitor herpesvirus genome. Interestingly, the HHV-6U51 gene product showed the closest sequence similarity to a cellularopioidreceptor.

A highly spliced gene at the right end of the UR of the genome has been characterized by analyzing a cDNA resulting from multiplesplicing, and it encodes the glycoprotein gp82/105 (50). Inthe case of strain GS, this gene contains 12 exons, and the singlelong ORF begins within exon 3 and ends in exon 12. In contrast,in strain HST, this gene contained eight or nine exons, and thesingle long ORF began within exon 2 and ended in exon 8 (61).The single long ORF encoding gp82/105 in strain GS is longer thanin strain HST. The differential splicing may play a role in thegeneration of various mRNA species that encode some protein componentsin the gp82/105 complex of the two variants. Furthermore, theamino acid sequence of each exon was divergent between variantsA and B (Table 1), and some monoclonal antibodies for gp82/105are variant A-specific neutralizing antibodies (49). Taken together,these findings suggest that the high degree of divergence in gp82/105may lead to differences in the cell tropism between variants AandB.

HHV-6 ORFs U20, U21, U23, U24, and U85 were predicted to encode glycoproteins. U20 and U85 encode homologs of the immunoglobulinE (IgE) C chain and OX-2 membrane antigen, both of which are membersof the Ig superfamily (10, 16). U24 of strain HST lacked anN-terminal signal sequence and may represent an exon (15).

Genes encoding glycoproteins were U12, U20, U21, U22, U23, U39, U48, U51, U72, U82, U85, U97, HN2, U98, U99, and U100. Amongthese, the ORFs with >90% identity were U20, U22, U39, U48, U51,U72, U82, and U85; ORFs with 80 to 90% identity were U12, U21,and U23; and those with 70 to 80% identity were U97, U98, U99,and U100. Of these glycoproteins, gp82/105 exhibited the mostdivergence.

(v) Capsid, tegument, and virus assembly proteins. Several ORFs of HHV-6 were homologous to herpesvirus genes encoding characterized or candidate structural proteins. Table1 shows that these include homologs of the major capsid protein(U57), minor capsid protein (U29), large tegument protein (U31),and virion proteins (U33, U34, U36, U50, U56, and U76) (7,15, 36, 44). Betaherpesvirus-specific and conserved structuralproteins are encoded by HHV-6 U11 (major antigenic phosphoprotein,pp100) (47, 48) and U54 (tegument transactivator), which arehomologs of HCMV UL32 (antigenic phosphoprotein, pp150) and UL82/U83(tegument transactivator, pp65/72K), respectively. The gene productsinvolved in DNA packaging and capsid assembly corresponded toHHV-6 U29, U30, U53, and U60/U66. The U53 gene encoded the protease/assemblyprotein (assemblin) and the scaffolding protein. Assemblin andscaffolding protein are derived from proteolytic cleavage andinternal initiation (15, 59, 69).

The genes U11, U29, U30, U31, U33, U34, U36, U49, U50, U53, U54, U56, U57, U60/U66, and U76 encoded viral structural proteins,and all except U11 and U54 showed >90% identity between strainsHST and U1102. In contrast, U11, a viral protein, and U54, a tegumenttransactivator, showed rather low identity (80.1 and 79.5%, respectively).These results suggest that the replication genes, except thosefor the U11 viral protein and the U54 tegument transactivator,may not be involved in the functional differences between variantsA andB.

Major repetitive elements. It has been observed that a remarkable divergence in the nucleotide sequence between strains JI and RK is present only inthe DR (38, 44). Similarly, between strains HST and U1102,marked differences were observed only in specific regions of theDR and the junction between the UR and DR. In the DRs of bothHST and U1102, the basic element of regions T1 and T2 (TAACCC)was related to human telomeric sequences (Fig. 2). These reiterationsconsisted of arrays of the basic element interspersed with 11types of human telomere-related elements, all hexonucleotides.In the case of strain HST, T1 was the longer reiteration, consistingof 54 copies of the telomeric element: 26 copies of the basictelomeric element and 28 copies of the human telomere-relatedelements. In contrast, T2 consisted of 26 copies of the basictelomeric element alone. In the case of strain U1102, T1 consistedof 54 copies of the telomeric element: 14 copies of the basictelomeric element and 40 copies of the related telomeric elements,most of which were also hexonucleotides but some of which werelarger. Furthermore, T2 of U1102 consisted of 59 copies of thebasic element alone. Thus, T2 of HST was half the size of thatof U1102, and T1 of HST contained more conserved telomeric elementsthan that ofU1102.

Repeat region R1 contains 52 copies of a dodecameric repeat element, consisting of its basic element (GAGGCCCTGCTG) and variants.However, it was difficult to determine the copy number of thedodecameric repeat element in R1 of U1102, because the reiterationsin R1 consist of remarkably variant elements. R1 was located inU86, the putative IE2 locus of HHV-6. R2 consisted of two typesof repeats, a 79- to 80-bp-long tandem repeat and a G/T repeat.The tandem repeat region in R2 of strain HST contained five copiesof a 79- to 80-bp repeat element, while that of U1102 containedtwo copies of imperfect repeats. R3 (Kpn repeat region) contained24 copies of tandemly repeated 104- to 107-bp-long elements and10 recognition sites for KpnI in strain HST (24), while R3 ofU1102 contained 28 copies of tandemly repeated 104- to 107-bp-longelements, all of which contained recognition sites for KpnI. Becauseof these differences, the region corresponding to the U92- andU93-homologous ORFs in strain HST was divided by six small ORFsand a small part of HN2. On the whole, the repeat elements ofstrain HST were more highly conserved than those of strainU1102.

Genetic divergence between HHV-6 variants. The marked divergence of variants A and B permitted the design of variant-specific oligonucleotide primers to detect DNA fragmentsthat differed in size between variants A and B HHV-6 DNA usingPCR. To analyze the genetic polymorphism of HHV-6 isolates, weexamined 14 different strains belonging to HHV-6 and one HHV-7strain, KHR (Fig. 3K). In this experiment, viral DNAs were extractedfrom human umbilical CBMCs that were infected with each virususing the protease K treatment method. PCR was performed as describedelsewhere (19), using the appropriate pairs of primers for U95,U86, U47, U11, and DR2, as shown in Fig. 3. No positive PCR productswere detected with uninfected cells or cells infected with otherhuman herpesviruses, including HSV-1 and -2, varicella-zostervirus, HCMV, and Epstein-Barr virus (data not shown). In the caseof HHV-7 (Fig. 3B, D, F, H, and J, lanes 15), however, among thegenes tested, a positive PCR product was detected only for theU47 gene, which was larger than those of HHV-6 (Fig. 3F). HHV-6DNA was detected in all 14 isolates by this method, and PCR productswere clearly separated into two groups in the case of the U95,U86, U47, and U11 genes: variants B and A showed fragments of342, 311, 362, and 168 bp and of 264, 209, 209, and 204 bp, respectively(Fig. 3K; also see Fig. 3B, D, F, and H). After amplificationof the DR2 genes, however, PCR products were clearly separatedinto three groups: 361 bp (variant B), 175 bp (U1102), and approximately265 bp (GS and DA) (Fig. 3J). These differences observed in variantA may be associated with the characteristic divergence of variantA viruses.

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FIG. 3. PCR typing of HHV-6. (A, C, E, G, and I) Schematic primary structures of ORFs U95, U86, U47, U11, and DR2 of strains HST and U1102. Positions and directions of the PCR primers are indicated by arrowheads at vertical lines. (B, D, F, H, and J) PCR amplification of DNAs from isolates 1 to 15 (K) of HHV-6 and HHV-7. Templates were purified from peripheral blood mononuclear cells infected with several laboratory strains and clinical isolates and were amplified with PCR primers (L). The products were fractionated by electrophoresis on 6% polyacrylamide gels and stained with ethidium bromide. The PCR products are indicated by arrowheads in panels B, D, F, H, and J. (K) Viruses used in the experiment. CFS, chronic fatigue syndrome.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have determined the complete DNA sequence of HHV-6 variant B strain HST, the causative agent of ES, and identified 115potential ORFs within the 161,573-bp contiguous sequence of theentire HHV-6 genome. When the sequence was compared with thatof the variant A strain U1102, some genes with remarkable differencesin amino acid identity wereidentified.

We conclude that the LT1, DR3, DR8, LJ1, RJ1, and DR3' ORFs probably do not encode proteins because LT1 and DR3 did not containpoly(A) signals, the ORFs of DR8, LJ1, and RJ1 contained telomericsequences, and DR3' contained a telomeric sequence between theORF and the poly(A) signal. As variant A-specific ORFs DR4, DR5,U78, U88, U92, and U93 were small and did not exhibit homologywith HHV-6B, HHV-7, other herpesvirus, and/or cellular genes,it is not likely that these genes encode functional proteins either.In contrast, HN1 and HN3 were variant B-specific genes and correspondedto exons of the IE1/IE2 and gp82/105 genes, respectively. We donot know whether HN2, DRHN1, and DRHN2 have homologous cellulargenes or encode functionalproteins.

All of the ORFs with <70% identity between the two variants were found to include deleted regions when the above-mentionedORFs were excluded from the comparison (Fig. 3 and reference 73).The remarkable differences except for U47 accumulated in someof the IE/regulatory genes (DR2, DR7, U86/90, U89/90, and U95)and may lead to characteristic differences between variants Aand B, although point mutations that we have not detected couldbe associated with these differences. The variation in IE proteinsmay be relevant to variant divergence because IE proteins controlthe temporal cascade of gene expression and are a second linein determining the cellular specificity of infection. Chou andMarousek (9) reported that variant B isolates segregate intotwo groups with even less divergence between them (92.6% identity).U89 derived from clinical isolates and strain Z29, which belongsto group 1, show more than 99.4% amino acid identity. In contrast,U89 of strain HST had 92.3% amino acid identity compared withstrain Z29 (Table 1). Clinical isolates, which belong to group2, have more than 99.4% amino acid identity compared to strainHST. These results suggest that strain HST belongs to group 2,although we do not know what function this divergence is associatedwith. In the case of U47, we cannot predict its function, buthomologous genes exist in HHV-7 and HCMV (U47 and UL74,respectively).

HHV-6 genes transcribed under IE conditions, that is, in the absence of prior protein synthesis, are U16/U17, U39, U42, U81,U89/U90, U91, and U94 ORFs (39). As some of these transcriptsare not translated under IE conditions, they may be regulatedin the posttranscriptional phase. If this is the case, some regulatorygene(s) likely plays an important role, and this mechanism wouldbe quite different from the known transcriptional regulation oftheherpesviruses.

In all sequenced herpesviruses, conserved glycoprotein genes encode gB, gH, gM, and gL, and the existence of neutralizingantibodies for gB and gH suggests that gB and gH/gL are essentialfor infection (62, 64). HSV-1 encodes an additional glycoprotein,gD, which recognizes cellular receptors (HveA, HveB, and HveC)(14, 40, 70), while HHV-6 encodes a different additionalglycoprotein, gp82/105, which is recognized by neutralizing antibodies(49). This finding suggests that gp82/105 may recognize a cellularreceptor(s). In addition, the gp82/105 glycoprotein of HHV-6 showedthe highest divergence in amino acid sequence between the twovariants. It is possible that gp82/105 leads to the differenceof cell tropism between variants A andB.

U83 of strain HST encodes a chemokine which functions as a chemoattractant for monocytes (76). Similarly, U83 of strainU1102 encodes a chemokine homolog, but it does not contain a signalpeptide sequence. Thus, U83 of strain U1102 may not be secretedand thus cannot exert its chemotactic activity. If U83 functionsas a chemoattractant in vivo, it is possible that HHV-6 can easilyspread through cell-to-cell infection, even in the presence ofneutral antibodies. Although we do not know whether the U83 geneproduct of HHV-6A contains a signal peptide, if it does not, wepredict that variant B viruses could easily spread in blood, whereasvariant A viruses shouldnot.

In analyzing the divergence in the functional proteins of HHV-6A and HHV-6B, we must consider that splicing would affect thegene layout and the level of relatedness between the HHV-6A andHHV-6B proteins. We have already obtained the splicing patternsof some mRNAs. These patterns are not as simple as predicted byMegaw et al. (38). For example, in the case of U79 and U80,there are a few more donor and acceptor splice sites than predictedby Megaw et al., and at least five kinds of mRNAs encoded by themcan be generated by alternative splicing (65). In the case ofIE1 and IE2, U90 is linked to U89 or U86 by alternative splicing.In the case of gp82/105, although there are donor and acceptormotifs, some signals on the mRNA appear not to be functional (50,61). We currently have no information about splicing in HHV-6A,except in the case of gp82/105. Further studies of splicing patternsshowing functional proteins may provide new insights into biologicaldivergence between HHV-6A and HHV-6B and molecular analysis oftheproteins.

Finally, we would like to point out that the divergence we have observed with IE/regulatory genes, gp82/105, and U83 betweenvariants A and B may lead to biological and pathogenic differencesbetween the two variants. Further functional studies of the genesshowing such remarkable divergence between variants may providenew insights into mechanisms for the molecular pathogenesis andcell tropism of HHV-6infection.

	ACKNOWLEDGMENTS

We are grateful to P. L. Ward for critical reading of and valuable comments on themanuscript.

This study was partly supported by a grant-in-aid for general scientific research from the Ministry of Education, Scienceand Culture ofJapan.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Osaka University Medical School C1, 2-2 Yamada-Oka Suita,Osaka 565-0871, Japan. Phone: 81-6-6879-3323. Fax: 81-6-6879-3329.E-mail: isegawa{at}micro.med.osaka-u.ac.jp.

Present address: Department of Virology, Research Institute for Microbial Diseases, Osaka University, 3-1 Yamada-Oka Suita,Osaka 565-0871,Japan.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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