The Primary Sequence of Rhesus Monkey Rhadinovirus Isolate 26-95: Sequence Similarities to Kaposi's Sarcoma-Associated Herpesvirus and Rhesus Monkey Rhadinovirus Isolate 17577

doi:10.1128/JVI.74.7.3388-3398.2000

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Journal of Virology, April 2000, p. 3388-3398, Vol. 74, No. 7
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The Primary Sequence of Rhesus Monkey Rhadinovirus Isolate 26-95: Sequence Similarities to Kaposi's Sarcoma-Associated Herpesvirus and Rhesus Monkey Rhadinovirus Isolate 17577

Louis Alexander, Lynn Denekamp, Amanda Knapp, Marcy R. Auerbach, Blossom Damania, and Ronald C. Desrosiers^*

New England Primate Research Center, Harvard Medical School, Southborough, Massachusetts 01772-9102

Received 27 September 1999/Accepted 21 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The primary sequence of the long unique region L-DNA (L for low GC) of rhesus monkey rhadinovirus (RRV) isolate 26-95 wasdetermined. The L-DNA consists of 130,733 bp that contain 84 openreading frames (ORFs). The overall organization of the RRV26-95genome was found to be very similar to that of human Kaposi sarcoma-associatedherpesvirus (KSHV). BLAST search analysis revealed that in almostall cases RRV26-95 coding sequences have a greater degree of similarityto corresponding KSHV sequences than to other herpesviruses. Allof the ORFs present in KSHV have at least one homologue in RRV26-95except K3 and K5 (bovine herpesvirus-4 immediate-early proteinhomologues), K7 (nut-1), and K12 (Kaposin). RRV26-95 containsone MIP-1 and eight interferon regulatory factor (vIRF) homologuescompared to three MIP-1 and four vIRF homologues in KSHV. Allhomologues are correspondingly located in KSHV and RRV with theexception of dihydrofolate reductase (DHFR). DHFR is correspondinglylocated near the left end of the genome in RRV26-95 and herpesvirussaimiri (HVS), but in KSHV the DHFR gene is displaced 16,069 nucleotidesin a rightward direction in the genome. DHFR is also unusual inthat the RRV26-95 DHFR more closely resembles HVS DHFR (74% similarity)than KSHV DHFR (55% similarity). Of the 84 ORFs in RRV26-95, 83contain sequences similar to the recently determined sequencesof the independent RRV isolate 17577. RRV26-95 and RRV17577 sequencesdiffer in that ORF 67.5 sequences contained in RRV26-95 were notfound in RRV17577. In addition, ORF 4 is significantly shorterin RRV26-95 than was reported for RRV17577 (395 versus 645 aminoacids). Only four of the corresponding ORFs between RRV26-95 andRRV17577 exhibited less than 95% sequence identity: glycoproteinsH and L, uracil DNA glucosidase, and a tegument protein (ORF 67).Both RRV26-95 and RRV17577 have unique ORFs between positions21444 to 21752 and 110910 to 114899 in a rightward direction andfrom positions 116524 to 111082 in a leftward direction that arenot found in KSHV. Our analysis indicates that RRV26-95 and RRV17577are clearly independent isolates of the same virus species andthat both are closely related in structural organization and overallsequence to KSHV. The availability of detailed sequence information,the ability to grow RRV lytically in cell culture, and the abilityto infect monkeys experimentally with RRV will facilitate theconstruction of mutant strains of virus for evaluating the contributionof individual genes to biologicalproperties.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Kaposi's sarcoma-associated herpesvirus (KSHV) is associated with classical and AIDS-related Kaposi's sarcoma (4, 6-8,23), as well as with primary effusion lymphoma (25, 36)and multicentric Castleman's disease (14, 31, 38). Sequenceanalysis of the KSHV genome (34) indicated that it is more closelyrelated to herpesvirus saimiri (HVS) than to other herpesvirusesand thus is assigned to the gamma-2 or rhadinovirus subgroup ofthe herpesvirus family (33). Investigation of the role of individualKSHV genes in replication and disease has been limited by thelack of a permissive cell culture system (13, 19, 32) andof an appropriate animalmodel.

A herpesvirus that can be grown lytically in cell culture was recently isolated from the peripheral blood of a rhesus monkey(animal 26-95) at the New England Regional Primate Research Center(12). Sequencing and BLAST search analysis of a 10.6-kbp fragmentof virion DNA revealed sequences corresponding to KSHV open readingframe (ORF) 7; intact genes for glycoprotein B (ORF 8), DNA polymerase(ORF 9), ORF 10, ORF 11, and viral interleukin-6 (vIL-6; ORF R2);and a partial gene for thymidylate synthetase (TS; ORF 70) (12).Based on these similarities in gene order and sequences this viruswas assigned to the rhadinovirus subgroup and named rhesus monkeyrhadinovirus (RRV) (12).

Recently, the primary sequence of an independent RRV isolate (isolate 17577) has been determined. RRV17577 sequences overthe same 10.6-kbp stretch were found to be colinear and closelyrelated to those from the original RRV26-95 isolate (37). Furthermore,the genome organization of RRV17577 was closely but not entirelycolinear with that of KSHV (37).

In this report, we reveal the complete primary sequence of the long unique region (L-DNA) of RRV26-95. The genomic organizationof RRV26-95 and sequence of individual ORFs contained within theL-DNA are compared to KSHV and RRV17577sequences.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Virus purification. RRV26-95 was grown in primary rhesus monkey fibroblasts in Dulbecco's modified Eagle's medium (Gibco, Grand Island, N.Y.)supplemented with 20% fetal bovine serum (Sigma, St. Louis, Mo.),2 mM L-glutamine, and penicillin-streptomycin (50 IU and 50 µg/ml,respectively), as previously described (12). Procedures forthe purification of virus have been previously detailed (11).Briefly, cells and debris were removed by low-speed centrifugationfollowing complete cell lysis. The supernatant was then filteredthrough a 0.45-µm-pore-size filter to remove any residual cellsand debris. The filtered supernatant was centrifuged for 3 h at17,000 rpm in a Sorvall type 19 rotor in order to pellet virus.Resuspended virus was fractionated by Sepharose 4B column chromatography,and virus contained in the void volume was used as a source ofvirion DNA forcloning.

Cloning of RRV26-95 DNA fragments. First, 10 µg of purified virion DNA in a 200-µl volume was sonicated for 10 s at 18% capacity in a 550 Sonic Dismembrator(Fischer Scientific, Medford, Mass.). Sonicated DNA was treatedwith T4 DNA polymerase (New England Biolabs, Beverly, Mass.) tocreate blunt ends and electrophoresed through 0.8% agarose, andDNA fragments of 0.5 to 1.0 kbp were isolated. Sonicated, purifiedDNA was inserted into the SmaI site of the pUC18 cloning vector(Pharmacia, Piscataway, N.J.). In addition, unsonicated DNA wasdigested with KpnI, EcoRI, SmaI, HindIII, and PstI restrictionenzymes (New England Biolabs). Then, 5.0- to 10.0-kbp restrictionfragments were isolated and cloned into either pUC18 (EcoRI, SmaI,and HindIII) or pSP72 (Promega) (KpnI and PstI) cloning vectors.As a control for the size of a stretch of repetitive DNA betweenORF 69 and R13 (Fig. 1), the EcoRI fragment vector (E6) was digestedwith RsaI and HaeIII enzymes. Restriction fragments were electrophoresedthrough 0.8% agarose, and 1.5-kbp RsaI and 1.3-kbp HaeIII fragments(Fig. 2) that were predicted to contain the repetitive sequencesof interest were isolated and inserted into the SmaI site of thepUC18 cloning vector. The plasmid clones described here were grownin XL-2 Blue MRF' ultracompetent cells (Stratagene, La Jolla,Calif.).

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FIG. 1. Alignment of ORFs of KSHV and RRV26-95. The different colors signify ORFs contained in KSHV and RRV26-95 that are conserved in the indicated herpesvirus subfamilies or subgroups. The square side of the symbol signifies the 5' end, and the pointed side of the symbol signifies the 3' end of the depicted ORFs. The ORFs are not drawn to scale.

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FIG. 2. The restriction digestion pattern of the RRV26-95 E6 clone. E6, an 11.0-kbp RRV26-95 restriction fragment clone that contains sequences from ORFs 66 to 71, was independently digested with HaeIII (lane 2) and RsaI (lane 3). Arrow 1 signifies the 1.5-kbp RsaI band (lane 3) and arrow 2 signifies the 1.3-kbp HaeIII band (lane 2) that contains highly repetitive sequences located between ORF 69 and R13 (Fig. 1) of RRV26-95. Lane 1 is a molecular weight marker, and the sizes of the marker bands are indicated at the left in thousands.

Assembly of RRV26-95 sequences. pUC18 clones were initially screened for insert DNA by HaeII digestion. The sequence of insert DNA from sonication clonesor the ends of restriction fragment clones was determined by usingM13 forward and reverse primers (Promega, Madison, Wis.) and aBig Dye Terminator Cycle Sequencing Ready Reaction kit (Perkin-ElmerCetus, Norwalk, Conn.). The ends of restriction fragment insertscloned into pSP72 were sequenced by using M13, T7, and SP6 primers(Promega). Sonication clones that contained a high G+C contentwere sequenced using a dGTP Big Dye Terminator Ready Reactionkit (Perkin-Elmer Cetus). Sequence data were edited using Sequencer3.0 software (Gene Codes Corporation) and assembled into contiguousoverlapping fragments (contigs) by using Sequencer and AssemblyLIGNsoftware (Kodak Lab Research, Rochester, N.Y.). Contig sequenceswere compared to sequences contained in GenBank by using BLASTXand assigned tentative positions to corresponding KSHV (34)and HVS (1) sequences. Gaps in sequence between contigs werefilled by PCR amplification of these sequences by using primersthat annealed near the end of contig sequences. The sequence ofthe majority of these gaps were then determined by using a seriesof custom primers to walk cloned DNA. For larger gaps, amplifiedDNA fragments were independently digested with two restrictionenzymes with four base recognition sites, AluI and RsaI (New EnglandBiolabs), and the resulting fragments were cloned into the SmaIsite of pUC18. The sequence of these fragments was determinedby using M13 forward and reverse primers as described above. Usingthese methods, we acquired the complete double-stranded sequenceof the L-DNA of RRV26-95. The sequence presented in this reportrepresents an average of 8.14 readings per base over the entireL-DNA.

Alignment and phylogenetic analysis of RRV26-95, RRV17577, and KSHV sequences. The positions of ORFs in RRV26-95 sequences were determined by using MacVector 5.0 software (Oxford Molecular Group, Campbell,Calif.). The sequences of these ORFs were aligned to RRV17577and KSHV ORFs using Gap Analysis software (Wisconsin GCG package,version 9.1; Oxford Molecular Group) and manually adjusted. Phylogenetictrees of RRV26-95, KSHV, and HVS ORF sequences were constructedby using PAUP* 4.0 software. A minimum of 200 bases of open sequencewas used to determine putative ORFs in the L-DNA of RRV26-95.

IL-6 rescue assay in B9 cells. RRV26-95 vIL-6 sequences were PCR amplified and inserted into the multiple cloning site located between the murine leukemiavirus (MuLV) long terminal repeat (L) and the simian virus 40(SV40) early promoter (S) of the vector LXSG (2). Thus, vIL-6transcription was driven by MuLV sequences, and transcriptionof the green fluorescent protein (G) was driven by SV40 sequences.The resulting clone and the control LXSG vector were electroporatedindependently into COS-1 cell cultures. Twenty-four hours later,green fluorescing cells were examined visually and by flow cytometry.Supernatants were collected from vIL-6-expressing and controlcultures. These samples were then incubated with the IL-6-dependentB9-cell line (5) for 48 h. At that time the viability of theB9 cells were tested using a cell proliferation kit(Promega).

Nucleotide sequence accession number. RRV26-95 nucleotide sequence data have been deposited in the GenBank nucleotide sequence database under the accession no.AF210726.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Genomic organization of RRV26-95. Sequence analysis of RRV26-95 virion DNA revealed 84 ORFs identifiable as herpesvirus genes within the 130,733 kbp that comprisethe L-DNA. The L-DNA had a G+C content of 52.1%. We have useda nomenclature for RRV26-95 ORFs that corresponds to that usedpreviously for KSHV ORFs (34). Beginning 513 bp upstream ofthe start of the R1 ORF, RRV26-95 contains repetitive sequenceelements lacking ORFs of significant length (data not shown).These data suggest that the L-DNA of RRV26-95 begins 513 bp upstreamof the start of the R1 ORF (10) and suggest that R1 is the leftmostgene in RRV26-95. Sequences 2,863 bp downstream of the RRV26-95ORF 75 initiate repeating elements absent of any ORFs of significantlength (data not shown). These sequences signify the 3' end ofthe RRV26-95 L-DNA. R15 is located in this 2,863-bp stretch ofsequence and is likely the rightmost gene in RRV26-95. The regionsnot included in the L-DNA are 65.0% G+C and are likely to representterminal repeat sequences. Included in the L-DNA sequences ofRRV26-95 are 39 genes that are common to all known herpesviruses(Fig. 1). In addition, beta- and gammaherpesvirus-specific ORFs18, 24, 45, and 66, as well as alpha- and gammaherpesvirus-specificORFs 21 (thymidine kinase), 60 (ribonucleotide reductase, small),and 65 are contained in RRV26-95 (Fig. 1). Gammaherpesvirus-specificORFs 27, 48, 49, 50, 52, 58, 59, 67.5, and 75, as well as gamma2-herpesvirus-specific ORFs 2 (dihydrofolate reductase; DHFR),4 (complement-binding protein; CBP), 70, 10, 11, and 73, and theTS gene common to gammaherpesviruses and the alphaherpesvirusvaricella-zoster virus, are contained in RRV26-95 (Fig. 1).

RRV26-95 contains a highly repetitive region located between R4 and vBcl-2 (ORF 16) (Fig. 1) that is 3,966 bp in length. Inthis region are two repeating elements: one of 26 bp that is repeated10 times and is 53.8% G+C and one of 25 bp that is repeated 27times and is 79.5% G+C (data not shown). The majority of the RRV26-95sequence in this region was determined from 10.6-kbp PstI (P5)and 10.5-kbp HindIII (H2) restriction fragment clones of virionDNA. The gap in sequence between these two clones was filled usingsequences from three clones derived from sonicated virion DNA.These experiments indicated that the size of the gap in sequencebetween P5 and H2 is 1,274 bp in length. Since we did not havea restriction fragment clone that spanned this region, we amplifiedthese sequences by using PCR primers that annealed to nonrepetitivesequences in P5 and H2 and used the amplified fragment for sizingand for sequencing. The resulting PCR fragment was of a size andsequence (data not shown) that indicated that the sequence representedby continuous restriction and sonication clones accurately representedthe RRV26-95 sequence between R4 and ORF 16. We observed one ORFin this region with sequences unique to RRV (seebelow).

Our analysis revealed another highly repetitive region that contained G+C-rich sequences between ORFs 69 and R13 (vFLIP) inRRV26-95 (Fig. 1). We have cloned an EcoRI restriction fragment(E6) of virion DNA that included sequences from ORF 66 to ORF71, and the size of this fragment (11 kbp) corresponded to thelength of the sequence determined for this region from overlappingclones derived from sonicated virion DNA. To further demonstratethat our determined sequence accurately represented RRV26-95 sequencesin this region, the E6 clone was digested with HaeIII and RsaIrestriction enzymes. Recognition sites for these enzymes flankedthe highly repetitive sequence region that is 1,127 bp in lengthand is 80.3% G+C. These sequences contained two repeating elements:one of 17 to 19 bp that is repeated 44 times and one of 31 bpthat is repeated 10 times (data not shown). The HaeIII and RsaIrestriction pattern of E6 agreed with the expected pattern basedon our determined sequence (Fig. 2). The 1.3-kbp HaeIII and 1.5-kbpRsaI digestion fragments (Fig. 2) were isolated and cloned intothe SmaI site of pUC 18. The sequence of these fragments was determinedand agreed with our sequence determination from overlapping fragmentsof sonicated virion DNA (data not shown), indicating that we accuratelydetermined the RRV26-95 sequences in this region. These analysesdemonstrate that the sequence between ORF 69 and R13 is 6,106bp. We observed RRV-unique ORFs in this region in both the rightwardand leftward directions without significant similarities to anyherpesviral or cellular sequences (seebelow).

Comparison of RRV26-95 and KSHV genomic organization and sequence. Our analysis indicates that the genomic organization of RRV26-95 is closely but not entirely colinear with that of KSHV (Fig.1). In most cases, RRV26-95 genes are in corresponding locationsand have the same polarity as corresponding KSHV genes (Fig. 1).However, several ORFs are contained in KSHV sequences that arenot contained in RRV26-95 sequences. These are K3 and K5 (bovineherpesvirus-4 immediate-early protein homologues), K7 (nut-1),and K12 (Kaposin) (Fig. 1). RRV26-95 contains only one vMIP-1homologue compared to three in KSHV (23), and RRV26-95 containseight homologues of vIRF compared to only four in KSHV (27,35) (Fig. 1). We have called the RRV26-95 vMIP-1 homologue R4and the vIRF homologues R9.1-R9.8 (Fig. 1, Table 1). Anotherdifference between RRV26-95 and KSHV is that the DHFR gene iscorrespondingly located near the left end of the genome in RRV26-95and the gamma-2 HVS, but in KSHV the DHFR gene is displaced 16,069nucleotides in a rightward direction in the genome (Fig. 1). Inall other cases, RRV26-95 genes are in corresponding locationsto and have the same polarity as corresponding KSHV genes (Fig.1).

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TABLE 1. Relatedness of ORFs in RRV26-95 to those in KSHV and RRV17577^a

By BLAST analysis, the level of similarity between RRV26-95 and KSHV for the 39 herpesvirus core gene sequences ranges froma low of 30.1% for ORF 28 to a high of 75.5% for ORF 9 (DNA polymerase)(Fig. 1, Table 1). The beta-gamma- (ORFs 18, 24, 45, and 66)and alpha-gamma- (ORFs 21, 60, and 65) herpesvirus-specific genescontained in RRV26-95 range in similarity to corresponding KSHVgenes from a low of 43.6% (ORF 45) to a high of 78.3% (ORF 60)(Table 1). Furthermore, similarities between RRV26-95 and KSHVgammaherpesvirus-specific genes (ORFs, 27, 48, 49, 50, 52, and75) range from 37.2% (ORF 27) to 65.8% (ORF 49) (Table 1). Inalmost all cases, beta-gamma-, alpha-gamma-, and gammaherpesvirus-specificORF sequences of RRV26-95 are more similar to KSHV than to otherherpesviruses (data not shown). DHFR is unusual in that RRV26-95DHFR more closely resembles HVS DHFR (74% similarity) than KSHVDHFR (55% similarity). With the exception of the DHFR gene, allhomologues are correspondingly located in KSHV and RRV26-95.

Our analysis revealed a number of ORFs that are common only to RRV and KSHV. Among these are ORF 1 (termed K1 in KSHV andR1 in RRV), vIL-6, vMIP, a series of interferon regulatory factors(vIRFs), vFlip, vOx-2, and a vIL-8 receptor (Fig. 1). These ORFsrange in similarity with corresponding KSHV ORFs from a low of30.6% (vIL-6) to a high of 42.8% (vMIP) (Table 1). Unlike K1sequences of some KSHV isolates which can display a high degreeof variability (41), the R1 sequences of RRV26-95 and RRV17577were 98% identical. Short ORFs that correspond in location tothe multiply spliced KSHV K8 (18, 40), K8.1 (17, 30) andK15 (9) genes were also observed in RRV26-95 and were calledR8, R8.1, and R15. Additional ORFs are located between RRV26-95ORFs 50 and 52 which are likely to contain additional R8, as wellas R8.1, sequences but these gene sequences cannot be determineddirectly from the primary sequence in the absence of detailedknowledge of splicing patterns. Downstream of ORF 75 sequences,RRV26-95 contains open sequences that correspond to open sequencesin RRV17577. These sequences are correspondingly located to themultiply spliced KSHV K15 gene (9, 30) and thus have beentermedR15.

Comparison of RRV26-95 and RRV17577 genomic organization and sequence. Our analysis indicates that RRV26-95 and RRV17577 have colinear genomic organizations (Table 1). Of the 84 ORFs in the RRV26-95L-DNA, 83 contain corresponding ORFs in RRV17577 and the overalldivergence within these sequences is only 2.24%. One exceptionis that RRV26-95 contains sequences for the herpesvirus core geneORF 67.5 (Fig. 1) which were not reported in the RRV17577 sequence(37) (Table 1). RRV26-95 ORF 67.5 (Fig. 1) is similar in size(86 amino acids [aa]) (Table 1) to corresponding KSHV sequences(80 aa) and contains several stretches of amino acids that areabsolutely conserved between RRV26-95 and KSHV (Fig. 3). Our inspectionof the RRV17577 sequence under accession no. AF083501 revealedan ORF 67.5 that was not noted by Searles et al. (37). It exhibited98.8% identity with ORF 67.5 of RRV26-95 (Table 1). The sequencesof RRV26-95 and RRV17577 also differ in a region in the L-DNAcontaining highly repetitive sequence located between vMIP-1 andvBcl-2 (Fig. 1) which is 288 bases (7%) shorter in RRV26-95 (3,966bp) than in RRV17577 (4,254 bp). In this region RRV26-95 containsone ORF which is 96% identical to corresponding RRV17577 sequences(see below). The corresponding region in KSHV is 8,313 bp andcontains the K4.1, K4.2, K5, K6, and K7 genes (Fig. 1) (26,34). Thus, both RRV26-95 and RRV17577 (37) do not containK4.2, K5, K6, and K7 gene sequences. RRV26-95 R4 has limited similarityto KSHV K4.1 but has high similarity to RRV17577 R3, which isthe name given to the corresponding gene in this isolate (Table1) (37). Despite the limited overall similarity, RRV26-95 R4contains four cysteine residues that are conserved among humanMIP homologues, K4, K6 (22, 34), and RRV17577 R3 (37), whichare characteristic of $beta$ -chemokines (data not shown). Our analysesalso demonstrate that the sequences between ORF 69 and R13 are6,106 bp for RRV26-95 compared to 6,314 bp for RRV17577. Thisregion contains highly repetitive, G+C-rich sequences which aresimilar to what was observed for RRV17577. The sequences in thisregion of both isolates do not contain sequences that are detectablysimilar to K12 (Kaposin) sequences (24) (Fig. 1).

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FIG. 3. Alignment of KSHV and RRV26-95 ORF 67.5. An alignment was constructed of KSHV (accession no. U75698) and RRV26-95 ORF 67.5 amino acid sequences by using CLUSTAL W software. Conserved residues are shaded in black.

Another exception to the overall similarity between RRV26-95 and RRV17577 is that the rhadinovirus-specific CBP sequencesare significantly shorter in RRV26-95 than was observed for correspondingsequences from RRV17577 (395 versus 645 aa) (Table 1) (37).RRV26-95 CBP sequences are contained in a 4.2-kbp KpnI restrictionfragment clone (K29) of virion DNA that spanned from just upstreamof R1 gene sequences to ORF 6 sequences (Fig. 1). This span ofvirion DNA matched the sequence determined from overlapping clonesderived from sonicated virion DNA and thus accurately representsRRV26-95 CBP sequence. We aligned RRV26-95 CBP amino acid sequenceswith RRV17577, KSHV, and HVS. Our analysis revealed that a regionof conservation exists among these sequences that begins at theN' termini of RRV26-95, KSHV, and HVS sequences which correspondsto amino acid 294 in the reported RRV17577 CBP open sequences(Fig. 4). Included in these sequences are 15 conserved cysteineresidues (Fig. 4). The sequences in this region of conservationare most similar between RRV26-95 and RRV17577 sequences (Fig.4). The N'-terminal 293 aa of the 645-aa RRV17577 CBP do not alignwith the other rhadinovirus CBP sequences depicted here. KSHVCBP is longer (550 aa) than RRV26-95 (395 aa) and HVS CBP (360aa) and contains C-terminal sequences downstream of the regionof conservation that also do not align with RRV or HVS sequences(Fig. 4).

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FIG. 4. Alignment of rhadinovirus CBP sequences. An alignment was constructed of CBP amino acid sequences from RRV17577 (accession no. AF083501), RRV26-95, KSHV (accession no. U75698), and HVS (accession no. X64346) by using CLUSTAL W software. The first 293 aa of RRV17577 CBP sequences did not align with the other rhadinovirus CBP sequences depicted here. Conserved cysteines are shaded in black. Deletion polymorphisms between sequences starting at amino acid 294 of RRV17577 CBP are indicated with dashes.

Reading frames unique to RRV. RRV26-95 was found to contain a number of reading frames not found in KSHV. A 102-aa reading frame is present between positions21,444 and 21,752. This reading frame which is unique to RRV (RU-1)corresponds in location to K4.1, K4.2, K5, K6, and K7 of KSHVbut has no homology to them or to any other KSHV sequences (Fig.1 and Table 2). A 102-aa reading frame with 96% identity is equivalentlylocated in RRV17577 (Table 2). Similarly, RRV26-95 contains aseries of ORFs between positions 110,910 and 114,899 in a rightwarddirection and between positions 116,625 and 111,082 in a leftwarddirection that have no similarity with KSHV but are reasonablyconserved when compared to RRV17577 (Table 2). These ORFs correspondin location (Fig. 1) but lack detectable similarity to the K12(Kaposin) gene. As described above, the RRV26-95 sequences inthis region contain two G+C-rich repeating elements: one of 17to 19 bp that is repeated 44 times and one that is 31 bp and isrepeated 10 times. The corresponding region of KSHV immediatelyrightward of the K12 gene contains two distinct 23-bp G+C-richrepeating sequences: DR1, which is 900 bp in length, and DR2,which is 370 bp in length (34, 35). Thus, although RRV lacksa Kaposin gene, it contains sequences in this region that arecomparable to KSHV.

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TABLE 2. Identity and similarity of RRV-unique (RU) ORFs^a

RRV26-95 ORF 73 sequences. RRV26-95 contains sequences for rhadinovirus-specific ORF 73 sequences (Fig. 1) which are 98% identical to RRV17577 sequences(Table 1). This ORF is significantly shorter (448 aa) than correspondingsequences in KSHV (1,162 aa) (34). The N' termini of RRV26-95and KSHV ORF 73 are both proline-rich (Fig. 5). Furthermore, BLASTsearch analysis revealed detectable similarity in the C'-terminalsequences of these genes (data not shown). Downstream of the proline-richsequences, KSHV ORF 73 sequences encode a long, highly acidicrepetitive domain (Fig. 5B) in contrast to RRV26-95 sequences,which only encode a short stretch of acidic residues in the correspondingregion of this gene (Fig. 5A). Thus, the difference in lengthbetween ORF 73 of RRV26-95 and KSHV is accounted for by the differencein the length of the acidic sequences.

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FIG. 5. The ORF 73 amino acid sequences of RRV26-95 (A) and KSHV (B) (accession no. U75698). Proline-rich sequences are shaded in black. The repetitive, acidic sequences in KSHV and the short stretch of acidic sequences in RRV26-95 are indicated in boldface.

Phylogenetic analysis of RRV26-95 vIRF sequences. RRV26-95 contains eight copies of vIRF homologues. These sequences have the highest similarity to the KSHV K9 vIRF homologue.To maintain consistency in nomenclature with KSHV, we have calledthe eight RRV26-95 vIRFs R9.1 to R9.8. K9 contains a proline-richmotif near its N terminus that is necessary for the interactionof K9 with p300 (M. Li, B. Damania, X. Alvarez, V. Ogryzko, K.Ozato, and J. U. Jung, submitted for publication). This interactionleads to the inhibition of the histone acetyltransferase activityof p300. Interestingly, none of the eight vIRF homologues in RRV26-95contains an N-terminal proline-rich motif (Fig. 6). Our analysisalso reveals that four of the R9 ORFs have 100% similarity andfour have a minimum similarity of 98.8% with the correspondingvIRF ORFs in RRV17577. A phylogenetic tree was built by usingthe R9 homologue sequences and was rooted to K9 sequences usingPAUP* 4.0 software (Fig. 7). These analyses demonstrate that R9.1branches with R9.5, R9.2 branches with R9.6, R9.3 branches withR9.7, and R9.4 branches with R9.8. There is very strong support(bootstrap values of 100%) for the branches separating these sequences.These data suggest that R9.5 to R9.8 arose from gene duplicationof R9.1 to R9.4 or vice versa. Parsimony analysis produced a treewith an identical topology (data not shown).

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FIG. 6. Alignment of N-terminal RRV26-95 and KSHV vIRF homologue sequences. An alignment was constructed of RRV26-95 R9.1 to R9.8 and KSHV K9 (accession no. U75698) N-terminal amino acid sequences by using CLUSTAL W software. The proline residues within the N-terminal region unique to KSHV K9 are shaded in black. Conserved residues among the K9 and R9 homologues are also shaded in black. Deletion polymorphisms are indicated with dashes.

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FIG. 7. Phylogenetic analysis of vIRF homologue genes of RRV26-95 and KSHV. CLUSTAL W software was used to align full-length R9.1 to R9.8 and K9 (accession no. U75698) amino acid sequences. The neighbor-joining method was used to generate this phylogeny by using PAUP* 4.0 software, with K9 sequences serving as the outgroup. Bootstrap values from 1,000 replications (repeated three times) are shown for each branch point.

Functional analysis of the RRV26-95 vIL-6 homologue. RRV26-95 sequences contain an ORF located immediately downstream of ORF 11 (Fig. 1) that is of similar size (Table 1) andin a corresponding location to the KSHV K2 gene (22, 27).We have termed this corresponding gene in RRV26-95 R2. Despitelimited overall similarity to K2 (Table 1), the R2 gene containsfour cysteine residues that are conserved in the IL-6 family ofcytokines (Fig. 8), and these cysteines have been shown to beimportant for the proper folding of the protein necessary forinteraction with the IL-6 receptor (21). To test functionality,we inserted RRV26-95 vIL-6 sequences into the vector LXSG (2)as described in Materials and Methods. In this construct, vIL-6transcription was driven by MuLV sequences and transcription ofthe green fluorescent protein was driven by SV40 sequences. Theresulting clone and the control LXSG vector were electroporatedindependently into COS-1 cell cultures, and green fluorescingcells were subsequently identified by flow cytometry. The parallelcultures were found to have been transfected with comparable efficiency(data not shown). Supernatants from these cultures were collectedand incubated with the IL-6-dependent cell line B9 (5). Cellproliferation assays revealed that B9 cells incubated with vIL-6supernatants were rescued in a dose-dependent manner in comparisonto B9 cells incubated with control supernatants (Fig. 9). Similarobservations have been made by others for KSHV K2 (22, 27)and RRV17577 R2 sequences (15).

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FIG. 8. Alignment of IL-6 sequences. An alignment was constructed of homologue IL-6 amino acid sequences from macaque (accession no. P51494), human (accession no. P05231), KSHV K2 (accession no. U75698), and RRV26-95 R2 by using CLUSTAL W software. Conserved cysteine residues that have been previously demonstrated to be necessary for IL-6 receptor binding are shaded in black. Deletion polymorphisms are indicated with dashes.

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FIG. 9. B9-cell rescue by RRV26-95 vIL-6. Twofold serial dilutions of supernatants from COS-1 cells transfected with a vector containing RRV26-95 vIL-6 or control vector were incubated with IL-6-dependent B9 cells. The rate of proliferation of B9 cells in the parallel cultures was determined by enzyme-linked immunosorbent assay with a cell proliferation kit.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Our analyses of RRV26-95 sequences demonstrate the similarity of this isolate to KSHV in genomic organization (Fig. 1) andin the sequence of individual ORFs (Table 1). BLAST search analysisrevealed that in almost all cases RRV26-95 coding sequences havea greater degree of similarity to corresponding KSHV genes thanto any other herpesvirus. All of the ORFs present in KSHV haveat least one counterpart in RRV26-95 except K3 and K5 (bovineherpesvirus-4 immediate-early protein homologues), K7 (nut-1),and K12 (Kaposin). These data suggest that these KSHV-specificgenes were acquired subsequent to the divergence of Asian andAfrican Old World primates. The repetitive, acidic domain in ORF73 of KSHV (Fig. 5) and the proline-rich domain in K9 (Fig. 6),absent in RRV26-95, may also have been acquired subsequent tothis divergence. DHFR is unusual in that it is located near theleft end of the genome in RRV26-95 corresponding in location toHVS DHFR and more closely resembles HVS DHFR (74% similarity)than KSHV DHFR (55% similarity). It seems likely that KSHV hasrearranged or reacquired the DHFR gene in the course of evolutionfrom Old World primate to humanrhadinoviruses.

Overall, RRV26-95 is very similar to RRV17577 both in sequence and in genomic organization. Furthermore, only four of 84 ORFsexhibited less than 95% sequence identity (Table 1). Despitethe high overall conservation between the two RRV isolates, somedifferences were noted between the two. Most notably, the CBPsequences in RRV17577 are significantly longer than in RRV26-95(Table 1). Alignment of these sequences with those of KSHV andHVS demonstrate that the N'-terminal 293 aa of RRV17577 encodingopen CBP sequence are not detectably similar to those of the RRV26-95,KSHV, or HVS CBP coding sequences (Fig. 4), whereas the 3'-most352 aa are similar to these rhadinovirus CBP coding sequences.Further work will be needed to determine whether the CBP sequencesof RRV17577 are unique. Although ORF 67.5 was not noted in thedescription of Searles et al. (37), it is present in the submittedsequence. These sequences are well conserved among herpesviruses,although their role in viral replication remains undefined. ORF67.5 sequences are 72% similar between RRV26-95 and KSHV (Table1).

The EBNA1 gene of Epstein-Barr virus (EBV) contains a long Gly-Ala repeat motif that plays a role in the inhibition of EBNA1-specificmajor histocompatibility complex class I antigen presentation(16). Recently, it has been shown that the EBNA1 gene of a rhesuslymphocryptovirus (20) contains a Gly-Ala repeat domain thatis considerably shorter than corresponding EBV sequence (3).This rhesus homologue does not maintain antigen presentation inhibitionactivity observed for the human homologue. KSHV ORF 73 sequencescontain a large, repetitive acidic motif (Fig. 5B), the functionof which remains to be determined. Conversely, RRV26-95 containsonly a short stretch of acidic residues in the corresponding regionof ORF 73 (Fig. 5A). It will be interesting to determine if therepetitive acidic motif contributes to the function of KSHV ORF73.

The K12 region is the most abundantly transcribed region in KSHV latent infection (35, 39). Recently, it has been demonstratedthat translation of the transcripts in this region is complex(35). The predominant translation product initiates at a CUGcodon and does not include K12 sequences but does include thetwo G+C-rich repeating units (DR1 and DR2) located immediatelyto the right of the K12 gene (34, 35). In the correspondingregion, RRV26-95 also contains two distinct G+C-rich repeatingelements that are comparable to the DR1 and DR2 sequences in KSHVbut does not contain sequences that are detectably similar toK12 (34, 35). It seems likely that RRV translation will alsobe complex in this region and may include sequences from the twoG+C-rich repeating elements, as well as the 12 ORFs located inthis region that are unique to RRV (Table 2).

The association of KSHV with Kaposi's sarcoma and other proliferative abnormalities has led to its intense study by numerouslaboratories. To date, these studies have been limited by thelack of a permissive, lytic system for KSHV (13, 19, 32)and by the lack of a direct animal model. This has precluded directdemonstration of the role of individual gene products in KSHVreplication, persistence, and disease. We have demonstrated herethat RRV26-95 is similar to KSHV both in genomic organizationand in the sequence of individual ORFs. Permissive growth of RRV26-95in rhesus monkey fibroblast cells (12) will facilitate geneticmanipulation of RRV sequences, including the engineering of pointmutations and deletions, as well as RRV recombinants that containmarker, cellular, or KSHV gene sequences. Study of the biologicalproperties of such mutant and recombinant viruses should provideinsight into the relative importance and role of individual genesto biologicalproperties.

	ACKNOWLEDGMENTS

We thank Jae Jung for valuable scientific discussions and comments; Yuan Chang for providing the B9 cell line; Kevin Clarke,Michelle Ethier, Susan Czajak, Daniel Silva, and Kim Deary forassistance; and Joanne Newton and Deborah Letourneau for manuscriptpreparation.

This study was supported by Public Health Service grants AI38131 andRR00168.

	FOOTNOTES

^* Corresponding author. Mailing address: New England Regional Primate Research Center, Harvard Medical School, One Pine HillDr., Southborough, MA 01772-9102. Phone: (508) 624-8040. Fax:(508) 624-8190. E-mail: ronald_desrosiers{at}hms.harvard.edu.

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Abstract
Introduction
Materials and Methods
Results
Discussion
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