Identification and Analysis of a Novel Heparin-Binding Glycoprotein Encoded by Human Herpesvirus 7

doi:10.1128/JVI.74.10.4530-4540.2000

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Journal of Virology, May 2000, p. 4530-4540, Vol. 74, No. 10
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Identification and Analysis of a Novel Heparin-Binding Glycoprotein Encoded by Human Herpesvirus 7

David Skrincosky,¹ Peter Hocknell,¹ Linda Whetter,¹ Paola Secchiero,²^,³ Bala Chandran,⁴ and Stephen Dewhurst¹^,⁵^,^*

Department of Microbiology and Immunology¹ and the Cancer Center,⁵ University of Rochester Medical Center, Rochester, New York 14642; Institute of Human Virology, University of Maryland at Baltimore, Baltimore, Maryland 21201²; Department of Morphology and Embryology, Human Anatomy Section, University of Ferrara, 44100 Ferrara, Italy³; and University of Kansas Medical Center, Kansas City, Kansas 66160⁴

Received 25 August 1999/Accepted 15 February 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Human herpesvirus 6 (HHV-6) and HHV-7 are closely related betaherpesviruses that encode a number of genes with no known counterpartsin other herpesviruses. The product of one such gene is the HHV-6glycoprotein gp82-105, which is a major virion component and atarget for neutralizing antibodies. A 1.7-kb cDNA clone from HHV-7was identified which contains a large open reading frame capableof encoding a predicted primary translational product of 468 aminoacids (54 kDa) with 13 cysteine residues and 9 potential N-linkedglycosylation sites. This putative protein, which we have termedgp65, was homologous to HHV-6 gp105 (30% identity) and containeda single potential membrane-spanning domain located near its aminoterminus. Comparison of the cDNA sequence with that of the viralgenome revealed that the gene encoding gp65 contains eight exons,spanning almost 6 kb of the viral genome at the right (3') endof the HHV-7 genome. Northern (RNA) blot analysis with poly(A)⁺ RNA from HHV-7-infected cells revealed that the cDNA insert hybridizedto a single major RNA species of 1.7 kb. Antiserum raised againsta purified, recombinant form of gp65 recognized a protein of roughly65 kDa in sucrose density gradient-purified HHV-7 preparations;treatment with PNGase F reduced this glycoprotein to a putativeprecursor of approximately 50 kDa. Gp65-specific antiserum alsoneutralized the infectivity of HHV-7, while matched preimmuneserum did not do so. Finally, analysis of the biochemical propertiesof recombinant gp65 revealed a specific interaction with heparinand heparan sulfate proteoglycans and not with closely relatedmolecules such as N-acetylheparin and de-N-sulfated heparin. Atleast two domains of the protein were found to contribute to heparinbinding. Taken together, these findings suggest that HHV-7 gp65may contribute to viral attachment to cell surfaceproteoglycans.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Human herpesvirus 6 (HHV-6) is a ubiquitous T-lymphotropic betaherpesvirus that was first discovered in 1986 (38) whichhas been etiologically linked to acute febrile illnesses in youngchildren, including exanthem subitum (35, 53). A closely relatedvirus, designated HHV-7 was discovered in 1990 (12) and hasalso been shown to be a ubiquitous, T-cell-tropic agent capableof causing exanthem subitum (22, 34, 46). Both viruses aretransmitted with high efficiency early in life, resulting in infectionof most children with both viruses by the age of 3 years (4,16, 47, 51, 54).

HHV-7 persists lifelong (like all other herpesviruses) and has been shown to establish a state of latency in peripheral bloodmononuclear cells (2). HHV-7's capacity for latency and itsability to specifically infect and kill CD4⁺ T cells (2, 12, 13) are properties which the virus shareswith the human immunodeficiency virus type 1 (HIV-1). Like HIV-1,HHV-7 binds to the CD4 molecule, and the virus uses CD4 as a componentof its host cell receptor (26). However, HHV-7 does not causeprogressive immunodeficiency disease and appears to establisha generally benign state of coexistence with its host. Furtherstudies of this virus may therefore shed light not only on themechanism whereby HHV-7 targets T lymphocytes but also on thebasis for the virus' apathogenicphenotype.

Herpesviruses encode as many as 10 or more glycoproteins targeted to the virion envelope. Many of these are involved in virusattachment to the cell surface or fusion of the viral envelopewith the plasma membrane (36). These viral glycoproteins mayalso serve as major targets for the host immune system. Informationabout HHV-7 glycoproteins is limited, although the virus is knownto encode homologs of the glycoproteins B, H, and L found in otherherpesviruses such as herpes simplex virus type 1 (HSV-1) (17,27-29, 41, 43). HHV-7 does not, however, encode a homolog ofthe essential HSV-1 receptor-binding glycoprotein D (6, 23,31, 49) or of the heparin-binding glycoprotein C (20, 21,45).

In the present study, we have focused our attention on the analysis of a novel glycoprotein which is unique to HHV-7 and HHV-6.In HHV-6, this molecule forms a complex (gp82-105) containingseveral polypeptides which share extensive amino acid identityand are thought to be derived from the same gene through differentialmRNA splicing (33). The gp82-105 complex is a major componentof the HHV-6 virion and represents a target for virus-neutralizingantibodies (32, 33), properties consistent with a possiblerole in virus attachment to, or penetration of, the hostcell.

The gene encoding HHV-6 gp105 spans several open reading frames (ORFs; U98 to U100) which are unique to HHV-6 and HHV-7 amongthe known human herpesviruses (33). We report here on the isolation,analysis, and characterization of a homologous gene in HHV-7.A 1.7-kb HHV-7 cDNA clone was identified, and a single major mRNAspecies of this same size (1.7 kb) was detected by Northern blotanalysis of poly(A)⁺ RNA from HHV-7-infected cells. A polyclonal antiserum raisedagainst the purified, recombinant protein product encoded by thiscDNA reacted with a glycoprotein of approximately 65 kDa (hereafterreferred to as gp65) that was present in lysates from virus-infectedcells and in highly purified HHV-7 virion preparations; this glycoproteinwas reduced in size to roughly 50 kDa upon digestion with N-glycanase(PNGase F). gp65-specific antiserum also neutralized the infectivityof cell-free virus inocula, providing additional support for thehypothesis that gp65 is a virion component. Finally, HHV-7 gp65was expressed in eukaryotic cells, and its biochemical propertieswere examined. Gp65 was found to interact specifically with heparinand heparan sulfate proteoglycans (and not with N-desulfated heparin,N-acetylheparin, or chondroitin sulfates A and C). These findingssuggest that HHV-7 gp65 may promote virus attachment to, or invasionthrough, cell surfaceproteoglycans.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

cDNA library. The cDNA library, which was generated from HHV-7_AL-infected SupT1 cells and cloned into the $lambda$ ZAPII vector (Stratagene, LaJolla, Calif.), has been described elsewhere (41). This librarywas screened with a digoxigenin-labeled (Boehringer Mannheim,Indianapolis, Ind.) DNA probe generated by PCR amplification ofHHV-7 genomic DNA with oligonucleotide primers corresponding tothe predicted location of the HHV-7 homolog of HHV-6 gp105 (29,33). Primers used were as follows: outer primers, 3733 (5'-AGAACTCATTGGGAGTGCGCGGAT)and 4350 (5'-TATGTCTCTCCAGGGTTCGATGGT); and inner primers, 2737(5'-ACTCTGTATCGTTGTTCG) and 3363 (5'-TCATCTCTTGGTCTTCTG). TheHHV-7 genomic coordinates of the final DNA probe were 140,225through 140,842 of HHV-7_JI.

5' RACE. Total RNA was isolated from HHV-7 infected SupT1 cells by using the RNeasy Kit (Qiagen, Valencia, Calif.). The RNA was subsequentlyDNase treated using RQ1 RNase-free DNAse I (Promega, Madison,Wis.) for 30 min at 37°C. An aliquot of the DNase-treated RNAwas analyzed on a 1.2% formaldehyde-agarose gel to assure integrity,and an additional aliquot of the DNase-treated total RNA was processedfor poly(A)⁺ RNA by using the Oligotex Kit (Qiagen). 5' rapid amplificationof cDNA ends (RACE) was performed by using the Boehringer Mannheim5'/3' RACE Kit on both the total RNA and the poly(A)⁺ RNA templates. Briefly, single-stranded cDNA was generated fromthe mRNA using gene specific primer PH1 (5'-CCGTATTGGTACATATCTTTATGAG;this corresponds to nucleotides 138942 to 138966 of HHV-7_JI).The cDNA was purified using the High Pure PCR Product PurificationKit (Boehringer Mannheim) and then poly(A) tailed using terminaltransferase and dATP. This material was then PCR amplified usingthe gene specific primer PH2 (5'-TTATATAATGCAGTTGCACCAT; thiscorresponds to nucleotides 138978 to 138999 of HHV-7_JI) and thecDNA amplification primer BMB (5'-GACCACGCGTATCGATGTCGACTTTTTTTTTTTTTTTTV;where V = A, C, or G). The PCR cycling protocol was 94°C for 2min, followed by 10 cycles of 94°C for 15 s, 55°C for 30 s, and72°C for 40 s, followed by 25 cycles of 94°C for 15 s, 55°C for30 s, and 72°C for 40 s (with a 20-s increase per extension cycle),followed by a final extension at 72°C. Two polymerase systemswere utilized for amplification: Taq polymerase (Promega) and,for enhanced fidelity, the Expand 20kb PCR System (BoehringerMannheim). Amplified products were analyzed on a 1.5% agarosegel and specific bands were gel isolated using the QIAquick GelExtraction Kit (Qiagen). Gel-purified products were then clonedinto the pGEM-T vector (Promega) and sequenced using the ABI PRISMDNA sequencing protocol (Perkin-Elmer, Foster City, Calif.). Thesequences obtained were analyzed using the BLASTalgorithm.

Northern (RNA) blot analysis. HHV-7 infected SupT1 cells were lysed using QiASHREDDER reagent, and total poly(A)⁺ RNA was isolated using an Oligotex mRNA isolation kit (Qiagen).RNA quality was verified by electrophoresis through a formaldehyde-containingagarose gel, and nucleic acids were transfered to a GenescreenPlus membrane (New England Nuclear, Boston, Mass.). The resultingblot was hybridized with a radiolabeled, single-stranded, gp65RNA probe that was generated using the T7-Riboprobe system (Promega).After overnight hybridization under conditions recommended bythe manufacturer, the blot was washed thoroughly and exposed toX-ray film (Eastman Kodak) at $-$ 70°C.

Baculovirus expression of gp65. A soluble derivative of HHV-7 gp65, bearing a carboxy-terminal polyhistidine epitope tag (His₆), was expressed in insect cellsby using a recombinant baculovirus expression vector. To do this,codons 23 to 468 of the gp65 cDNA were subcloned into the pMelBacBvector (Invitrogen, Carlsbad, Calif.) in frame with the honeybeemellitin signal sequence. Subcloning of gp65 sequences was achievedby PCR amplification with Pfu DNA polymerase and using the oligonucleotideprimers BALA1, (5'-tcgaggatcctGAAAAAGCACGCACGGCAATAACT) and BVB1(5'-agcgtcgacctagtggtggtggtggtggtgACCACCCATAACATTTTGTAACT)(lowercase letters denote nonviral sequences, including the translationstop codon [in boldface], while uppercase letters represent gp65-specificsequences; underlined residues are the restriction sites, anditalicized residues correspond to the His₆ epitope tag). Aftercloning into pMelBacB, recombinant baculovirus was generated usingthe Bac-N-Blue system (Invitrogen). PCR analysis was used to verifythe presence of HHV-7 insert sequences in plaque-purified virusclones, and protein expression from these clones was verifiedby immunoblot analysis of culture supernatants from virus-infectedHigh Five cells (Invitrogen) by using a His₆-specific monoclonalantibody (Qiagen). For subsequent biochemical studies (e.g., heparinbinding), medium containing the expressed proteins was collected,centrifuged to remove debris, and concentrated using Centricon-30microconcentrators (Amicon, Bedford, Mass.). Protein concentrationswithin these samples were determined using the Bio-Rad ProteinAssayReagent.

Generation of mouse antisera to gp65. Supernatants from High Five insect cells that were infected with a gp65-expressing baculovirus vector were collected and dialyzedextensively against 50 mM sodium phosphate-0.5 M NaCl (pH 8.0).His₆-tagged gp65 was then purified using nickel-agarose (Qiagen),eluted with imidazole, and analyzed by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE). Protein preparations containingonly a single detectable band upon Coomassie blue staining ofSDS-polyacrylamide gels were used for injection into a BALB/cmouse (11 µg per injection, delivered subcutaneously in Freundcomplete adjuvant). After initial protein injection, the animalwas boosted by a second protein injection in Freund's incompleteadjuvant (29 days after the initial inoculation), and serum wascollected 21 days thereafter. The specificity of this antiserum(and the corresponding prebleed serum sample) was then assessedby immunoblot analysis using His₆-tagged gp65 as atarget.

Generation of rabbit antisera to gp65. The preparation of the immunogen was similar to that described above, except that the recombinant His₆ tagged gp65 proteinwas bound to nickel-nitriloacetic acid (NTA)-agarose beads (Qiagen)which were then pelleted, washed extensively with 50 mM sodiumphosphate-0.5 M NaCl-20 mM imidazole (pH 8.0), and resuspendedin phosphate-buffered saline (PBS) as a 75% gel slurry. A 1-mlaliquot of this material (i.e., His₆-tagged gp65 protein, boundto nickel-NTA-agarose beads) was then mixed with an equal volumeof Freund's complete adjuvant and injected into a 6-month-oldmale New Zealand White rabbit (Cocalico Biologicals, Reamstown,Pa.). The rabbit received a boost injection in Freund's incompleteadjuvant 1 week after the initial immunization and once a monththereafter for four consecutive months. Each immunization deliveredapproximately 15 to 50 µg of His₆-tagged HHV-7 gp65. Ten daysafter the last boost, the rabbit was sacrificed by exsanguination,and serum was collected. Like the mouse antiserum, this antiserumreacted specifically with gp65 upon immunoblot analysis of bothpurified recombinant gp65 and highly purified HHV-7 virion preparations,while the matched preimmune serum did not react with gp65 (datanotshown).

Immunoblot analysis of HHV-7 virions. A lysate of sucrose density gradient-purified HHV-7 virions (strain H7-4) was obtained from Advanced Biotechnologies, Inc.(Columbia, Md.). Aliquots of this material were then separatedby SDS-PAGE, transferred to nitrocellulose, and analyzed by immunoblotanalysis, using the mouse antiserum directed against gp65. Theantiserum was used at a dilution of 1:100, and bound antibodieswere detected using a horseradish peroxidase (HRP)-conjugatedanti-mouse antibody and chemiluminescent reagents (ECL; Amersham-Pharmacia,Piscataway, N.J.). In some experiments, the viral lysate was digestedwith N-glycanase (Peptido-N-Glycosidase F [PNGase F]; Oxford GlycoSciences,Wakefield, Mass.) for 14 h at 37°C (2.5 U of enzyme/5 µg of virallysate) prior to separation by SDS-PAGE and immunoblotanalysis.

Radioimmunoprecipitation. To determine whether gp65 was expressed in HHV-7-infected SupT1 cells, 6 × 10⁶ infected or uninfected cells were radiolabeled for 18 h in 10ml of methionine- and cysteine-free Dulbecco modified Eagle medium(Gibco, Grand Island, N.Y.) supplemented with 5% dialyzed fetalbovine serum, 2 mM glutamine, and 25 µCi of Expre³⁵S³⁵S-Protein Labeling Mix (New England Nuclear) per ml. After labeling,the cells were collected into pellets and lysed in 1.5 ml of PBScontaining 0.1% Triton X-100, 1 mM phenylmethylsulfonyl fluoride,and 2 µg of pepstatin per ml, 7.5 µg of bestatin per ml, and 5µg each of antipain, aprotonin, leupeptin, and soybean trypsininhibitor per ml. After 30 min, insoluble cellular debris wasremoved by centrifugation. Each lysate was divided into two equalaliquots, and these were incubated with gp65-specific mouse antiserumor preimmune serum, respectively, for 2 h at 4°C. Protein A-Trisacrylbeads (Pierce, Rockford, Ill.) were then added to the samplesand, following a 1-h incubation, the beads were pelleted, washedwith PBS-0.1% Triton X-100, and boiled in SDS-PAGE sample buffer.Eluted proteins were resolved by electrophoresis on a 12.5% polyacrylamidegel. The gel was fixed, soaked in Amplify reagent (Amersham),dried, and subjected tofluorography.

HHV-7 gp65 mutagenesis. The 1,338-bp fragment of HHV-7 gp65 cDNA (codons 23 to 468) previously cloned in the s-pIG vector (Novagen, Madison, Wis.)was used a substrate for mutagenesis. Two putative heparin-bindingdomains were targeted for mutagenesis, which was performed byalanine substitution using the QuikChange mutagenesis kit(Stratagene).

Mutant clones were designated as follows: M1 (¹⁵⁹ARHRWERR¹⁶⁶ $right-arrow$ ¹⁵⁹AAAAWERR¹⁶⁶), M2 (¹⁸⁴FKKMRS¹⁸⁹ $right-arrow$ ¹⁸⁴FAAMRS¹⁸⁹), and M12 (both mutations introduced into the same DNA clone).The oligonucleotide primers used in the M1 and M2 mutagenesisreactions were, respectively, as follows: DM1 (5'-AGCCTGGTTTTGTTCCCTGCTgctgctgcTTGGGAAAGACGTGAGCAATA)and DM1R (5'-TATTGCTCACGTCTTTCCCAAgcagcagcAGCAGGGAACAAAACCAGGCT);and DM2 (5'-TTACAGATACGCGCAGATTTTgctgctATGCGTAGCTACAGCGGAATA)and DM2R (5'-TATTCCGCTGTAGCTACGCATagcagcAAAATCTGCGCGTATCTGTAA).The uppercase letters denote authentic HHV-7 sequences, whilethe lowercase letters denote mutated residues. After mutagenesis,which was conducted according to the manufacturer's protocol,a short restriction fragment spanning the entire mutated region(a 476-bp HindIII/SphI fragment; bp 353 to 820) was excised andsubstituted for the corresponding region within the pMelBacB-gp65-(His₆)expression construct. The final clones were then sequenced toverify the presence of the desired mutations (and the lack ofany additional changes), and recombinant baculovirus expressionvectors encoding the mutated derivatives of HHV-7 gp65 were generated(seeabove).

Analysis of heparin-binding by gp65. Culture supernatants from High Five insect cells infected with the gp65-(His₆)-expressing baculovirus recombinant (10 µg ofprotein) were prepared in 500 µl of PBS containing 0.1% TritonX-100, in the presence or absence of 350 µg of various competitorglycosaminoglycans (heparin; heparan sulfate; chondroitin sulfatesA, B, and C; N-acetylheparin; and de-N-sulfated heparin; all ofthese reagents were obtained from Sigma, St. Louis, Mo.). Afterbeing mixed for 1 h at 4°C, 100 µl of a 50% slurry of heparin-acrylatebeads (Sigma) equilibrated in PBS-0.1% Triton X-100 (containingapproximately 35 µg of immobilized heparin) was added. Sampleswere mixed for 2 h at 4°C, after which the beads were pelletedand unbound material was removed. The beads were subsequentlywashed five times with 1 ml of PBS-0.1% Triton X-100, and boundmaterial was eluted by boiling the beads in 50 µl of SDS-PAGEsample buffer. Heparin-bound and unbound material was resolvedon SDS-12.5% polyacrylamide gels and electroblotted onto nitrocellulosemembranes (AmershamPharmacia).

To detect the gp65-(His₆) protein, nitrocellulose membranes were blocked overnight at 4°C in PBS-0.05% Tween 20 containing5% nonfat dry milk; blots were probed with a Penta-His monoclonalantibody (Qiagen) in PBS-0.05% Tween 20-2% milk, followed by HRP-conjugatedsheep anti-mouse immunoglobulin (Amersham Pharmacia). Bound antibodieswere detected with ECL Detection Reagents (Amersham Pharmacia),and biotinylated molecular weight markers (Bio-Rad, Hercules,Calif.) were visualized by using HRP-streptavidin (AmershamPharmacia).

Virus neutralization experiments. Filtered (0.45 µm [pore size]) infectious supernatant obtained from HHV-7-infected SupT1 cells was used. The procedures forHHV-7 propagation in the SupT1 CD4⁺ lymphoblastoid T-cell line and the preparation of virus stockshave been previously described (26, 40, 42). For the virusneutralization assay, the viral inoculum was preincubated for60 min at room temperature with rabbit anti-gp65 immune and preimmunesera. SupT1 cells were then incubated with the treated or untreatedviral stocks (500 µl of virus per 250,000 cells; multiplicityof infection [MOI] of approximately 0.1) and seeded in culturein 24-well plates (Costar, Corning, N.Y.). Infection was monitoredby light microscopic examination (for the detection of syncytia)and by indirect immunofluorescence staining at 48 and 72 hpostinfection.

GenBank accession number. The sequences described here have been deposited with GenBank (accession no. AF198085).

	RESULTS

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Identification and analysis of the HHV-7 gp65 gene. A digoxigenin-labeled HHV-7 DNA probe corresponding to the HHV-6 gp105 gene (33) was used to screen a library of cDNAs fromHHV-7_AL-infected SupT1 cells, cloned into the $lambda$ ZAPII vector (41).After several rounds of screening, a total of six positively hybridizingclones were selected for further analysis. Plasmids were excisedfrom the lambda phage vector and subjected to DNA sequence analysisby using oligonucleotide primers derived from the T3 and T7 promoterelements which flank the inserted cDNAs in this vector. Five ofthe six cDNA clones were found to contain common sequences, derivedfrom ORFs U98 to U100 on the complementary strand of the HHV-7genome (clones 1111, 2113, 3115, 4117, and 6119). Thus, theseclones corresponded to sequences with homology to the HHV-6 gp105gene (33). The sixth clone (clone 1116) was derived from a differentgene, encoded on the opposite strand of the viral genome (27,29). The splicing patterns and sequence contents of these variouscDNAs are summarized in Table 1.

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TABLE 1. HHV-7 cDNA clones which hybridize to a HHV-6 gp105 DNA probe^a

Complete sequence analysis of clone 1116 revealed that it corresponds to a spliced mRNA encoding the viral DR1 gene product(27, 29). As shown in Table 2, the splicing pattern detectedin this cDNA was identical to that predicted by Megaw and colleagues(27), with the addition of a short upstream exon (noncoding).The major ORF contained within this cDNA clone is predicted toencode a protein of 344 amino acids. This is somewhat shorterthan the DR1 gene product predicted by Megaw and coworkers, afinding presumably due to the differences in the length of thedirect repeats (DRs) of HHV-7_AL (which served as the source ofour cDNA clones) versus the DRs of HHV-7_RK (27).

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TABLE 2. Exon positions within HHV-7 cDNA clone 1116

Since we were interested in the HHV-7 homolog of HHV-6 gp105, we directed the remainder of our attention toward the analysisand characterization of the remaining five cDNA clones. In vitrotranscription and translation (IVTT) of these cDNAs, using T7RNA polymerase, showed that a detectable protein product was generatedonly in the case of clone 4117 (data not shown). DNA sequencingof this clone was therefore performed. Sequence analysis usingthe GCG software package (8) revealed the presence of a singlelarge ORF of 1,404 nucleotides within the cDNA. The putative initiationcodon (ATG) at nucleotide 174 conformed to Kozak's rules for translationalstart sequences (25), having an A at position $-$ 3 and a G atposition +4; this ATG was preceded by an upstream, in-frame stopcodon at nucleotide 153. The ORF stop codon (TAA) was locatedat nucleotide 1578, and a potential polyadenylation signal (AATAAA)was detected between residues 287 and 292 on thecDNA.

The ORF contained within this cDNA clone was predicted to be capable of encoding a primary translational product of 468 aminoacids (approximately 54 kDa), with a pI of 7.25, 13 cysteine residues,and 9 consensus N-linked glycosylation sites. Overall, this putativeprotein product exhibited 30% amino acid identity and 39% similarityto its counterpart in HHV-6, as determined by using the GAP algorithm(8). Analysis of predicted protein hydrophilicity suggestedthat the putative protein is likely to possess a noncleaved hydrophobicsignal sequence and membrane anchor of approximately 23 aminoacids, making it a tail-anchored class II membrane glycoprotein(48) like its HHV-6counterpart.

Our predictions with respect to protein size and posttranslational modification were experimentally verified by IVTT of thecDNA insert from clone 4117. This resulted in the production ofa protein of approximately 50 kD, which was converted to a moleculeof roughly 65 kDa upon the addition of canine microsomes to theIVTT reaction (data not shown), suggesting that the protein isglycosylated in vivo. In light of these findings, we designatedthis novel viral glycoproteingp65.

Splicing and transcription of HHV-7 gp65. Comparison of the nucleotide sequence from the gp65-encoding cDNA with that of the HHV-7 genome revealed that the gene encodinggp65 contains eight exons, spanning almost 6 kb of the viral genome(Table 3). The first exon (nucleotides 1 to 170) maps to theviral terminal direct repeats and is predicted to be noncoding,due to the presence of an upstream, in-frame stop codon at nucleotide153, relative to the putative initiator methionine within thecDNA (nucleotide 174). All other exons in the cDNA correspondto sequences present at the right (3') end of the unique longsegment of the viral genome. Each of the exons contained withinthis cDNA clone showed 100% nucleotide identity with the correspondinggenomic regions from both HHV-7 strain JI and HHV-7 strain RK,emphasizing the highly conserved nature of HHV-7 genomes (27).

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TABLE 3. Exon positions within the gene that encodes gp65 in the cDNA and the HHV-7_JI genome sequences

As noted above, four additional cDNA clones (clones 1111, 2113, 3111, and 6119) also contained fragments of the U98 throughU100 viral ORFs (Table 1). Clone 1111 was found to possess thesame predicted coding capacity as clone 4117 (i.e., the same ATGand TAA codons at nucleotide positions 138,998 and 137,080 ofthe HHV-7_JI genome, respectively), while clones 2113 and 3115were determined to contain exons 3 to 8 and 4 to 8 of the gp65gene, respectively. These clones may therefore represent incompletecDNA clones that lack an intact 5' end (Table 1). Finally, clone6119 had a very similar organization to that of clone 4117 andalso spanned exons 2 to 8 of the gp65 gene, terminating at aninternal oligonucleotide A stretch within exon 8. The first in-frameATG codon in this clone was the same as that found in clone 4117.However, exon 1 of clone 6119 was derived from a different regionof the viral direct repeats (nucleotide positions 141,154 to 141,070of the HHV-7_JI genome) compared to exon 1 of clone 4117. Sequenceanalysis of this clone suggested that this new upstream regiondid not change the predicted translation product of the cDNA relativeto clone4117.

Since the 5' ends of the gp65-encoding cDNA clones 4117 and 6119 were different, we undertook to map the 5' end(s) of thegp65-encoding mRNA(s) by using 5'-RACE analysis. In order to dothis, we generated oligonucleotide primers corresponding to the5' end of exon 2 of the cDNA clones 4117 and 6119 (this regionis conserved in both of these cDNAs; see Fig. 1). We then usedthis primer to perform PCR amplification of cDNA fragments correspondingto the 5' end(s) of the gp65 mRNA(s); the PCR-derived cDNA fragmentswere then cloned and subjected to sequenceanalysis.

The sequencing results revealed a somewhat unexpected pattern of RNA 5' ends (see Table 4). In no case did we generate cloneswith structures identical to clones 4117 or 6119. Rather, sevenof eight clones analyzed were found to extend into the HHV-7 DRbefore undergoing a splicing event (Table 4). As a consequence,these clones all contained the pac1 motif and a short array oftelomeric repeat sequences (TRSs) derived from the 5' end of theright DR. This splicing pattern may have been missed in the cDNAclones due to the instability of the viral TRS motifs in Escherichiacoli (unpublished data). One additional RACE clone lacked thepac1-TRS elements but contained portions of exon 1 from clone6119, as well as portions of exon 1 from clone 4117 (Table 4).

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TABLE 4. Exon positions within 5'-RACE clones derived from gp65 mRNAs

These findings confirmed the heterogeneous nature of the transcripts encoding HHV-7 gp65, at least in terms of their 5' ends(this information is summarized in schematic form in Fig. 1).However, all eight of the 5'-RACE clones were found to containan in-frame stop codon located upstream of the putative initiatormethionine codon identified in cDNA clones 4117 and 6119. Thus,the expected protein-coding capacity of the RACE-derived cDNAclones was found to be identical to that of gp65 cDNA clone 4117.

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FIG. 1. Schematic summary of cDNA clones and 5'-RACE clones analyzed in this study. The upper portion of this figure shows a schematic representation of the right end of the HHV-7 genome, including the DR and the pac1 and TRSs located at the boundary between the DR and the right end of the unique portion of the viral genome. All genomic positions are relative to the JI strain of HHV-7 (in kilobases). The lower portion of the figure shows the structure of the various cDNA and 5'-RACE clones which are described in this study. These include cDNA clone 1116, which corresponds to a putative DR1 cDNA, as well as five cDNAs (intact and partial) which correspond to putative gp65-encoding cDNAs. In all cases, the location of the first methionine within the major ORF of each cDNA is indicated by an asterisk, while the location of the stop codon is located by an open box. Note that the DR1 cDNA is of opposite polarity to the gp65 cDNAs. Finally, the structures of the 5'-RACE clones are shown in the box at the bottom of the figure. A total of eight RACE clones were sequenced, and their structures were found to fall into three groups (as shown). Seven of the eight clones were found to extend into the HHV-7 DR before undergoing a splicing event. As a consequence, these clones all contained the pac1 motif and a short array of telomeric repeat sequences. One RACE clone lacked the pac1-TRS elements but contained portions of the exon 1 from cDNA clone 6119, as well as portions of exon 1 from cDNA clone 4117. Importantly, all of the RACE clones contained an in-frame stop codon upstream of the first methionine codon (the stop codon is not marked on this figure, but the methionine codon is denoted by an asterisk). Thus, the predicted protein-coding capacity of these RACE-derived clones appears to be identical to that of gp65 cDNA clone 4117.

Northern (RNA) blot analysis of poly(A)⁺ RNA, using a single-stranded radiolabeled RNA probe generated from plasmid clone 4117,revealed the presence of a single major mRNA species of approximately1.7 kb in poly(A)⁺ RNA from virus-infected SupT1 cells but not in control (virus-negative)SupT1 cells (Fig. 2). Larger, but less-abundant RNA species werealso detected, which may represent splicing intermediates or theproducts of differential mRNA splicing, as has been suggestedfor the HHV-6 gp105 gene (33). Hybridization of the same RNApreparations with a double-stranded radiolabeled DNA probe correspondingto the HHV-7 glycoprotein B gene (43) resulted in the detectionof a single major hybridizing species of roughly 3.4 kb (Fig.2). This finding is consistent with a previously published report(41). The detection of higher-molecular-weight hybridizationsignals with the gB probe (Fig. 2) has also been described andwas previously attributed to larger RNA precursors (41).

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FIG. 2. Northern blot analysis of HHV-7 gp65. Poly(A)⁺ RNA was isolated from HHV-7-infected SupT1 cells (I) or from uninfected cells (U), and equal amounts of RNA were then subjected to denaturing agarose gel electrophoresis and transferred to a nylon membrane. The blot was hybridized with a single-stranded, radiolabeled RNA probe corresponding to HHV-7 gp65 or to a radiolabeled DNA probe corresponding to HHV-7 gB (as indicated) and exposed to X-ray film. Shown is a photograph of the resulting autoradiogram. The arrows denote the major RNAs which hybridized to the probes used; sizes were estimated on the basis of the mobility of RNA molecular weight markers (Life Technologies, Inc.).

Biochemical analyses of HHV-7 gp65. Inspection of the predicted amino acid sequence of gp65 revealed the presence of two putative heparin-binding Cardin-Weintraubconsensus motifs (7): (i) at amino acid 159, ARHRWERR (thismotif is of the type XBBBXXBX, where B is a basic amino acid andX represents any amino acid); and (ii) at amino acid 184, FKKMRS(this is of the type XBBXBX). In light of the presence of thesesequence motifs, we theorized that gp65 might be capable of bindingto cellular glycosaminoglycans. To test this hypothesis, we generateda recombinant baculovirus expression vector which encoded a solublederivative of HHV-7 gp65 bearing a carboxy-terminal histidinetag (His₆) that could be used to facilitate protein detectionand purification. Culture supernatants from insect cells infectedwith this baculovirus vector were reacted with heparin-acrylatebeads, in the presence or absence of an excess of various glycosaminoglycans.After an extensive washing, the beads were boiled in SDS-PAGEsample buffer, and the eluted gp65-(His₆) was detected by immunoblotanalysis using the His₆-specific monoclonal antibody. Representativeresults are presented in Fig. 3A.

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FIG. 3. HHV-7 gp65 exhibits heparin-binding activity. (A) Insect cell culture supernatants containing soluble recombinant gp65-(His₆) were incubated with heparin-acrylate beads in the absence (lanes 5 and 10; negative control) or presence of an excess amount of various glycosaminoglycans, including heparin (lanes 4 and 9; positive control), heparan sulfate (lane 1), N-acetylheparin (lane 2), de-N-sulfated heparin (lane 3), and the chondroitin sulfates A, B, and C (lanes 6, 7, and 8, respectively). After a washing, the beads were boiled in SDS-PAGE sample buffer, and eluted proteins were separated by electrophoresis on an SDS-12.5% polyacrylamide gel and transferred to nitrocellulose. Immunoblot analysis was then conducted using an anti-His₆ monoclonal antibody and a chemiluminescent detection system (see Materials and Methods). (B) Lysates from COS-1 cells that were transiently transfected with a plasmid expression construct encoding lacZ-(His₆) were incubated with heparin-acrylate beads in the absence (lanes 2 and 4) or presence (lanes 1 and 3) of heparin. Heparin-acrylate-bound material (lanes 1 and 2) and unbound material (lanes 3 and 4) were then subjected to immunoblot assay using an anti-His₄ monoclonal antibody. Lane 5 represents a positive control in which the transfected cell lysate was directly submitted to immunoblot analysis without prior treatment with heparin-acrylate beads. In both panels, the numbers on the left represent molecular mass markers (in kilodaltons), while the arrows denote gp65-(His₆) (A) and lacZ-(His₆) (B), respectively. The experiments were repeated three times (A) or twice (B) with similar results.

The data show that gp65-(His₆) bound to heparin-acrylate beads (Fig. 3A, lanes 5 and 10) and that this binding was competitivelyinhibited by the addition of excess soluble heparin to the reactionmixture (Fig. 3A, lanes 4 and 9). Heparan sulfate was also foundto be an effective competitor for gp65 binding to heparin-acrylatebeads (Fig. 3A, lane 1), while chondroitin sulfates A and C failedto inhibit the interaction of gp65 with heparin-coated beads (Fig.3A, lanes 6 and 8), as did chemically modified heparin derivativeswhich lack the N-sulfate group (N-acetylheparin and de-N-sulfatedheparin; Fig. 3A, lanes 2 and 3,respectively).

Previous studies have noted that histidine, while basic, is not enriched in heparin-binding peptide sequences (5). Furthermore,long stretches of basic amino acids are uncommon in heparin-bindingproteins (14), and histidine itself appears to be a rather poorheparin binder (5, 14). Nonetheless, we performed additionalcontrol studies to verify experimentally that the His₆ epitopepresent in our recombinant HHV-7 gp65 did not bind to heparin.To do this, cells were transfected with an expression vector encodinga recombinant derivative of E. coli $beta$ -galactosidase (LacZ) thatcontains an C-terminal His₆ epitope tag (pcDNA3.1MycHisLacZ+;Invitrogen). Lysates from these transfected cells were then reactedwith heparin-acrylate beads, and the bound (Fig. 3B, lanes 1 and2) or unbound (Fig. 3B, lanes 3 and 4) fractions were analyzedby immunoblot analysis using a His₄-specific monoclonal antibody;binding experiments were conducted in the presence (Fig. 3B, lanes1 and 3) or absence (Fig. 3B, lanes 2 and 4) of excess solubleheparin. As is evident from the data presented in Fig. 3B, thepresence of the C-terminal His₆ epitope tag in E. coli lacZ didnot confer the ability to bind to heparin on the protein. Furthermore,radiolabeled gp65 produced in baculovirus without the histidinetag was also shown to bind to heparin-acrylate beads (data notshown).

Having concluded that gp65-(His₆) interacts specifically with heparin but not with several other closely related glycosaminoglycans,we proceeded with experiments designed to define the regions withingp65 that might contribute to heparin binding. First, short biotinylatedpeptides were synthesized (ADFKKMRSYS and PARHRWERRE) that correspondedto the two putative heparin-binding motifs within HHV-7 gp65 (residues182 to 191 and residues 158 to 167, respectively). The two HHV-7peptides both bound to radiolabeled heparin, while an irrelevantpeptide from adenovirus type 7 fiber protein (GSFNPVYP) did notdo so (data not shown). Furthermore, this binding could be inhibitedby the addition of excess cold heparin but not by the additionof N-acetylheparin or de-N-sulfated heparin, suggesting that thebinding was specific (data notshown).

In order to confirm that the putative heparin-binding domains within gp65 were functional in the context of the intact protein,site-directed mutagenesis studies were conducted. Three mutantsof gp65 were constructed: (i) M1 (¹⁵⁹ARHRWERR¹⁶⁶ $right-arrow$ ¹⁵⁹AAAAWERR¹⁶⁶), (ii) M2 (¹⁸⁴FKKMRS¹⁸⁹ $right-arrow$ ¹⁸⁴FAAMRS¹⁸⁹), and (iii) M12 (which contains both of these mutations). Thesemutants were expressed with a C-terminal (His₆) epitope tag ininsect cells, using the baculovirus system, and tested for theirability to bind to heparin-acrylate beads. As shown in Fig. 4,each of the individual gp65 mutants exhibited decreased bindingto heparin (binding was approximately 40 to 50% of the wild-typelevel in both cases; Fig. 4B). The double mutant, which lacksboth of the putative heparin-binding motifs, exhibited an evenlower level of binding (approximately 28% of the wild-type level;Fig. 4B). In all cases, binding was competed away entirely inthe presence of an excess of soluble heparin (data not shown).

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FIG. 4. Analysis of heparin-binding by mutated derivatives of HHV-7 gp65. Mutated derivatives of HHV-7 gp65 were constructed, and the proteins were then expressed in insect cells, with a C-terminal (His₆) epitope tag. Heparin-binding by the proteins was then assessed (see Fig. 3 for methods). (A) The results of one representative heparin-binding experiment are shown. Lanes are as follows: 1 to 4, input protein (directly loaded onto the gel and then probed by immunoblotting with the anti-His₆ monoclonal antibody); 5 to 8, protein bound to heparin-acrylate beads and then analyzed by immunoblotting with the anti-His₆ monoclonal antibody. Wild-type gp65-(His₆) was analyzed in lanes 1 and 5, while mutant derivatives of gp65-(His₆) were analyzed in the other lanes (lanes 2 and 6, M1; lanes 3 and 7, M2; lanes 4 and 8, M12). (B) Results from four independent heparin-binding experiments (including the one shown in panel A) were densitometrically quantitated and normalized in terms of input protein loaded (as detected by the anti-His₆ immunoblot assay). The amount of the mutant proteins which bound to heparin-agarose beads was then expressed as a percentage of heparin-binding by wild-type gp65-(His₆), and mean binding values were plotted in the figure; bars represent the standard error of the means.

Taken together, the data presented in Fig. 4 show that each of the two putative heparin-binding domains within HHV-7 gp65contributes to the ability of the intact protein to bind to heparin.However, it also appears that other protein domains may contributeto heparin-binding, since the double mutant still binds detectablyto heparin. Additional studies will be required to define theseadditional heparin-binding regions withingp65.

HHV-7 gp65 is expressed in virus-infected cells and is present within highly purified virion preparations. The results of the heparin-binding experiments suggested the possibility that HHV-7 gp65 might play a role in the processof virus binding or entry into host cells. This would be consistentwith the fact that soluble heparin can block HHV-7 infection (43).We therefore decided to examine whether gp65 was present in HHV-7-infectedcells and in purified virion preparations derived from such cells.To do this, a polyclonal mouse antiserum was raised against thebaculovirus-derived gp65-(His₆) protein. The specificity of thisantiserum was then verified by performing enzyme-linked immunosorbentassay and immunoblot analyses using purified recombinant gp65-(His₆)(data notshown).

The immune serum was used to conduct immunoprecipitation analyses of radiolabeled lysates from HHV-7-infected SupT1 cells,and control (uninfected) SupT1 cells. As shown in Fig. 5, theantiserum reacted specifically with a single major protein speciesof approximately 65 kD in the virus-infected cell lysates. Theimmune serum did not react with lysates from uninfected SupT1cells (Fig. 5), and the matched preimmune serum failed to reactwith lysates from either virus-infected or uninfected SupT1 cells(data not shown). The reactivity of the gp65-specific mouse antiserumwith the recombinant gp65-immunoglobulin (gp65-Ig) fusion proteinis shown in Fig. 6A. As expected, the corresponding preimmuneserum failed to react with this recombinant gp65-Ig fusion protein(Fig. 6A).

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FIG. 5. HHV-7 gp65 is expressed in HHV-7-infected cells. A murine polyclonal antiserum was raised against the baculovirus derived gp65-(His₆) protein and used to perform immunoprecipitation analysis of radiolabeled cell lysates from HHV-7-infected SupT1 cells (SupT1/HHV7) and from uninfected SupT1 cells (SupT1). The immune antiserum reacted with a single major protein species of approximately 65 kDa (indicated by the arrow). The preimmune serum did not react with this protein (data not shown; see also Fig. 6).

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FIG. 6. HHV-7 gp65 is present within highly purified HHV-7 virion preparations. A murine gp65-specific polyclonal antiserum (see Fig. 5) was used to perform immunoblot analyses of sucrose density gradient-purified HHV-7 virion preparations. (A) The immune antiserum (I) or its preimmune counterpart (P) was reacted with a purified gp65-Ig fusion protein (this fusion protein contained amino acid residues 23 to 325 of gp65, fused in frame to the Fc portion of human immunoglobulin G, contained in the signal pIg-Tail vector; Novagen, Inc.). As shown by the asterisk, only the immune antiserum reacted with the gp65-Ig protein (ca. 70 kDa). (B) The immune antiserum (I) or its preimmune counterpart (P) was reacted with a lysate of sucrose density gradient-purified HHV-7 virions. The arrow denotes the specific reactivity of the immune antiserum with a protein doublet of roughly 65 kDa. (C) The HHV-7 virion lysate was subjected to extensive digestion with N-glycanase (PNGase F) prior to immunoblot analysis with the immune antiserum (N). In control experiments, the lysate was incubated in reaction buffer alone (i.e., no PNGase was added) under the same conditions (B), or the lysate was analyzed directly, without prior treatment in vitro ( $-$ ). The arrow denotes the position of HHV-7 gp65, while the filled circle shows the size of the product of PNGase digestion of this molecule (ca. 50 kDa).

The gp65-specific antiserum was next used to perform an immunoblot analysis of a lysate of sucrose density gradient-purifiedHHV-7 virions. As shown in Fig. 6B, the immune antiserum reactedwith a protein doublet of approximately 65 kDa in the virion preparation(denoted by the arrow), which was not detected by the preimmuneserum. Finally, to confirm that gp65 was glycosylated, we conductedin vitro deglycosylation experiments using N-glycanase (PNGaseF). As shown in Fig. 6C, enzymatic deglycosylation of the HHV-7virion preparation reduced gp65 to a putative precursor form ofroughly 50 kDa (denoted by the filledcircle).

The findings shown in Fig. 6 strongly suggest that gp65 is a component of HHV-7 virions. However, further analysis revealedthat the highly purified virion preparation contained not onlyviral proteins (gp65) but also cellular membrane components (e.g.,transferrin receptor and CD3; data not shown). This raised thepossibility that viral nonstructural proteins might also be presentwithin the these virion preparations. We therefore performed additionalexperiments to confirm that gp65 is indeed a component of presentin HHV-7virions.

Immunoelectron microscopy studies using the mouse polyclonal antiserum have been unsuccessful to date, and we therefore resortedto more-indirect experiments, designed to test if gp65-specificantisera might neutralize the infectivity of HHV-7. These studiescould not be performed using the gp65-specific mouse antiserum,since they required relatively large volumes of serum. Thus, itwas necessary to generate a polyclonal rabbit antiserum directedagainst HHV-7 gp65 using the recombinant baculovirus-derived gp65-(His₆)immunogen (see Materials and Methods). After verifying that thisserum reacted specifically with recombinant forms of gp65 [gp65-Igand gp65-(His₆)] and with native gp65 from virion preparations(data not shown), we then used it to conduct virus neutralizationexperiments, using high-titer, cell-free virus inocula. Resultsfrom a representative neutralization experiment are shown in Fig.7. It can be readily appreciated that the gp65-specific immuneantiserum efficiently blocked virus-induced cytopathic effects(syncytium formation) in SupT1 cells (Fig. 7C and E), whereasthe corresponding preimmune serum had no effect on virus-inducedsyncytium formation (Fig. 7D and E). This finding was corroboratedby immunofluorescence analysis of viral antigen expression inthese cultures (data not shown) and was confirmed in a replicateexperiment. Taken together with the data in Fig. 6, these findingsstrongly suggest that HHV-7 gp65 is indeed a virion glycoprotein,with a molecular size that is consistent with the predicted sizeof the product of our cloned cDNA species.

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FIG. 7. A gp65-specific antiserum neutralizes virus infectivity. An infectious, cell-free stock of HHV-7 was generated, and preincubated for 60 min at room temperature with a diluted aliquot of rabbit polyclonal antiserum raised against the baculovirus-derived gp65-(His₆) protein. SupT1 cells were then incubated with the treated virus preparation (MOI of ~0.1), and infection was monitored by light microscopic examination of syncytium formation at 72 h following virus infection. Panels: A, negative control (uninfected SupT1 cells, with no added virus); B, positive control (SupT1 cells infected with HHV-7 in the absence of any antiserum); C and E, SupT1 cells exposed to the virus-containing inoculum and preincubated with gp65-reactive immune serum at a dilution of either 1:25 or 1:100, respectively; D and F, SupT1 cells exposed to the virus-containing inoculum and preincubated with preimmune rabbit serum at a dilution of either 1:25 or 1:100, respectively. Note the presence of extensive syncytia in panels B, D, and F, but not in the panels in which the virus inoculum was treated with the gp65-specific serum (panels C and E). Magnification, ×250.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Foa-Tomasi and colleagues reported that seven glycoproteins were immunoprecipitated from HHV-7-infected cells by human serumantibodies, with molecular masses of 100, 89, 82, 67, 63, 53,and 43 kDa (11). While the genes which encode these glycoproteinshave not been determined, it is likely that at least some of themmay correspond to glycoproteins B, H, and L. These glycoproteinshave been found to have molecular masses of roughly 100 to 110kDa (17, 43), 80 to 90 kDa (28, 41), and 33 to 37 kDa(28), respectively. Thus, either or both of the 67- and 63-kDaglycoproteins previously identified by Foa-Tomasi and coworkerscould conceivably represent products of the gp65 gene (ORFs U98to U100). This would be consistent with the size of the virionform of gp65 which we detected here. Further studies will be requiredto determine if this is indeed the case. However, we have beenable to show that antibodies present in sera from HHV-7-positivechildren recognized Ni-agarose-purified gp65-(His₆) in an immunoblotassay, while the protein was not detected by sera from HHV-7-negativechildren (data notshown).

The predicted size of HHV-7 gp65, at 468 amino acids, is considerably shorter than its counterpart in HHV-6 (650 amino acids)(33). This difference is consistent with the compressed structureof the right (3') end of the unique long segment of the HHV-7genome compared to that of HHV-6 (15, 27, 29). Furthermore,two ORFs which contribute to the HHV-6 gp105 gene (ORFs 96 and97) and which map to this genomic region are lacking in HHV-7.

Like HHV-6 gp105, HHV-7 gp65 is encoded by a highly spliced mRNA. Splice donor and acceptor consensus sequences were identifiedin the viral genome at the boundaries of each of the exons (Table3), and the overall pattern of splicing was very similar to thatpredicted by Megaw and colleagues, based on an analysis of theHHV-7 genome. These authors suggested that the gp65 gene fromHHV-7_RK, which they termed ORF U100, contain 10 exons (27).The first seven of these exons were found in the present gp65cDNA (clone 4117, Table 3). However, two differences were observedbetween Megaw's prediction and our experimentally determined findings.First, the putative splice donor at the end of exon 7 was notused in this cDNA, which therefore lacks the final three downstreamexons (8 to 10) that were predicted by Megaw et al. (27). Second,an unanticipated, noncoding, upstream exon was found in our gp65cDNA, which was derived from a position within the viral DRs.This suggests that the promoter element for this gene may be locatedwithin the DRs, a finding that was supported by our 5'-RACE analysis.It also raises the possibility that the gene could be expressedfrom the DR_L element, following genome circularization withinthe infectedcell.

Our Northern blot analyses revealed that the major gp65 RNA species present in virus-infected cells was approximately 1.7kb in length (i.e., the same size as our cDNA clone). This suggeststhat the cDNA clone obtained is full length. This interpretationis reinforced by the fact that the apparent molecular size ofthe in vitro-translated protein product of the cDNA clone (~50kDa) was very similar to the observed size of the enzymaticallydeglycosylated form of virion gp65 (also ~50 kDa). The fact thatour gp65-specific antiserum reacted with two distinct gp65 isoformsof roughly 65 kDa in virion preparations may suggest some variationin the posttranslation modification of gp65, since only a singleprotein species was detected after PNGasetreatment.

Predictive analysis of the gp65 sequence revealed the presence of two putative heparin-binding motifs and prompted us to speculatethat gp65 might represent a heparin-binding glycoprotein. Thishypothesis was experimentally validated by using a soluble recombinantderivative of gp65. This glycoprotein was found to interact specificallywith heparin and heparan sulfate proteoglycans but not with de-N-sulfatedheparin or chondroitin sulfates A and C. The selectivity of gp65for heparin and heparan sulfate, but not for chondroitin sulfatesA and C, strongly suggests that this binding interaction is specificfor heparan sulfate proteoglycans (37, 44). This interpretationis supported by the fact that gp65 binding to heparin was dependenton N-sulfation, since neither N-acetylheparin nor de-N-sulfatedheparin could competitively inhibit gp65 binding to heparin-acrylatebeads.

The functional relevance of the two putative heparin-binding sites within HHV-7 gp65 was confirmed by using two complementaryapproaches. First, short peptides corresponding to the two domainswere synthesized and examined for their ability to bind to radiolabeledheparin. Second, site-directed mutations were introduced intothe intact gp65 protein at each of the putative heparin-bindingmotifs (individually or in combination). Heparin-binding by thesefull-length mutant derivatives of gp65 was then examined. Thetwo assay systems yielded similar and consistent findings. Eachof the two domains examined was found to be capable of bindingto heparin in a functional assay, and both domains were foundto contribute to heparin binding by the intact protein. The dataalso suggest that at least one more region must contribute toheparin binding by HHV-7 gp65, since a mutated version of theprotein that lacks both of the predicted binding sites was foundto retain the ability to bind to heparin (albeit with reducedefficiency). Precedent for this exists, in that the pseudorabiesvirus glycoprotein C has been shown to contain multiple discreteunits that can function independently of one another to mediatebinding to heparan sulfate proteoglycans (HSPGs) (10).

In addition to gp65, HHV-7 also encodes a second glycoprotein which has been found to bind to cell surface heparan sulfateproteoglycans (glycoprotein B), and soluble heparin has been shownto inhibit viral infection and syncytium formation in the SupT1T-cell line (43). The presence of two heparin-binding glycoproteinswithin a single virus is not unexpected. Indeed, all well-studiedhuman alpha- and betaherpesviruses contain at least two glycoproteinswhich bind to HSPGs: a glycoprotein B homolog (found in all alpha-and betaherpesviruses [reviewed in reference 30]) and a memberof either the gC family (for alphaviruses [19, 21]) or gC-II(for human cytomegalovirus [24]). Presumably, the presence oftwo heparin-binding glycoproteins within the same virus indicatesthe importance of cell surface proteoglycans as receptors forviral attachment (reviewed in reference 37). In addition, itis possible that HHV-7 gB and gp65 may exhibit differences intheir relative affinity for distinct cell surface heparan sulfateproteoglycans, as do HSV-1 gB and gC (18).

It is intriguing to note that HHV-6A (GS) gp105 also contains three putative heparin-binding motifs of the type XBBXBX (⁹⁴LKRVKA⁹⁹, ¹⁹⁷MRRLKP²⁰², and ⁶¹⁹PRKLRC⁶²⁴), whereas the predicted protein products of two recently identifiedHHV-6B (Z29) gp105 cDNAs (B. Chandran, unpublished data) containonly a single consensus heparin binding motif of the type XBBXBX(²⁹¹VHHDRP²⁹⁶ in the Z29 U100 ORF from the complete genome of HHV-6B strainZ29). The single putative heparin-binding motif within HHV-6Bgp105 is likely to be weak at best, since histidine, while basic,is not enriched in heparin-binding peptide sequences (5) andappears to be a rather poor heparin binder (5, 14). Thus,it is conceivable that differences in the interaction of HHV-6gp105 glycoproteins with cell surface heparan sulfate proteoglycanscould contribute to differences in the observed host cell tropismof HHV-6A and HHV-6B. Additional experiments will be requiredto test thishypothesis.

In conclusion, the findings reported here suggest that HHV-7 encodes two heparin-binding glycoproteins which may play a rolein the process of virus infection (glycoprotein B and gp65 [identifiedfor the first time here]). These molecules may contribute to thevirus' ability to attach to and enter human cells, including salivarygland cells (3, 9, 50, 52) and primary human CD4⁺ T lymphocytes (12). Further studies of HHV-7 and its encodedglycoproteins may shed light on the biological properties of thisubiquitous human virus and may provide insights that could contributeto the development of gene delivery vehicles capable of targetingCD4⁺ T cells (12) and/or the salivary gland (1, 39).

	ACKNOWLEDGMENTS

We thank Caroline Hall and Renee Norton for providing HHV-7 stocks and virus-infected SupT1 cells, John Frelinger and RickWillis for assistance with the generation of mouse antisera, RobertRose and Chris Lane for assistance with baculovirus propagationand preparation, George Kampo and Jack Maniloff for preparationof oligonucleotides and for performing DNA sequence analyses,and Bo Wisdom (Kansas University Medical Center Protein Core Facility)for preparation and purification of synthetic peptides. We alsothank Robert Linhardt and Ishan Capila for assistance with theidentification of putative heparin-binding elements within HHV-7gp65 and Greg Williams and James Whitman of Advanced Biotechnologies,Inc., for expert advice andassistance.

This work was supported by NIH grants to S.D. (R21 AI34231 and KO4 AI01240), by NIH Training Grants T32 CA09363 and T32 AI07362to D.S. and P.H., and by Telethon grant 279/bi to P.S.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology and Immunology, University of Rochester Medical Center,601 Elmwood Ave., Box 672, Rochester, NY 14642. Phone: (716) 275-3216.Fax: (716) 473-2361. E-mail: stephen_dewhurst{at}urmc.rochester.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Baum, B. 1995. Salivary gland repair. Adv. Dental Res. 9:22[Medline].

2. Berneman, Z. N., D. V. Ablashi, G. Li, M. Eger-Fletcher, M. S. Reitz, Jr., C. L. Hung, I. Brus, A. L. Komaroff, and R. C. Gallo. 1992. Human herpesvirus 7 is a T-lymphotropic virus and is related to, but significantly different from, human herpesvirus 6 and human cytomegalovirus. Proc. Natl. Acad. Sci. USA 89:10552-10556[Abstract/Free Full Text].

3. Black, J. B., N. Inoue, K. Kite-Powell, S. Zaki, and P. E. Pellett. 1993. Frequent isolation of human herpesvirus 7 from saliva. Virus Res. 29:91-98[CrossRef][Medline].

4. Black, J. B., T. F. Schwarz, J. L. Patton, K. Kite-Powell, P. E. Pellett, S. Wiersbitzky, R. Bruns, C. Muller, G. Jager, and J. A. Stewart. 1996. Evaluation of immunoassays for detection of antibodies to human herpesvirus 7. Clin. Diagn. Lab. Immunol. 3:79-83[Abstract].

5. Caldwell, E. E., V. D. Nadkarni, J. R. Fromm, R. J. Linhardt, and J. M. Weiler. 1996. Importance of specific amino acids in protein binding sites for heparin and heparan sulfate. Int. J. Biochem. Cell Biol. 28:203-216[CrossRef][Medline].

6. Campadelli-Fiume, G., M. Arsenakis, F. Farabegoli, and B. Roizman. 1988. Entry of herpes simplex virus 1 in BJ cells that constitutively express viral glycoprotein D is by endocytosis and results in degradation of the virus. J. Virol. 62:159-67[Abstract/Free Full Text].

7. Cardin, A. D., and H. J. Weintraub. 1989. Molecular modeling of protein-glycosaminoglycan interactions. Arteriosclerosis 9:21-32[Abstract/Free Full Text].

8. Devereux, J., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.

9. Di Luca, D., P. Mirandola, T. Ravaioli, R. Dolcetti, A. Frigatti, P. Bovenzi, L. Sighinolfi, P. Monini, and E. Cassai. 1995. Human herpesviruses 6 and 7 in salivary glands and shedding in saliva of healthy and human immunodeficiency virus positive individuals. J. Med. Virol. 45:462-468[Medline].

10. Flynn, S. J., and P. Ryan. 1996. The receptor-binding domain of pseudorabies virus glycoprotein gC is composed of multiple discrete units that are functionally redundant. J. Virol. 70:1355-1364[Abstract].

11. Foa-Tomasi, L., E. Avitabile, L. Ke, and G. Campadelli-Fiume. 1994. Polyvalent and monoclonal antibodies identify major immunogenic proteins specific for human herpesvirus 7-infected cells and have weak cross-reactivity with human herpesvirus 6. J. Gen. Virol. 75:2719-2727[Abstract/Free Full Text].

12. Frenkel, N., E. C. Schirmer, L. S. Wyatt, G. Katsafanas, E. Roffman, R. M. Danovich, and C. H. June. 1990. Isolation of a new herpesvirus from human CD4⁺ T cells. Proc. Natl. Acad. Sci. USA 87:748-752[Abstract/Free Full Text].

13. Frenkel, N., and L. S. Wyatt. 1992. HHV-6 and HHV-7 as exogenous agents in human lymphocytes. Dev. Biol. Stand. 76:259-265[Medline].

14. Fromm, J. R., R. E. Hileman, E. E. Caldwell, J. M. Weiler, and R. J. Linhardt. 1997. Pattern and spacing of basic amino acids in heparin binding sites. Arch. Biochem. Biophys. 343:92-100[CrossRef][Medline].

15. Gompels, U. A., J. Nicholas, G. Lawrence, M. Jones, B. J. Thomson, M. E. Martin, S. Efstathiou, M. Craxton, and H. A. Macaulay. 1995. The DNA sequence of human herpesvirus-6: structure, coding content, and genome evolution. Virology 209:29-51[CrossRef][Medline].

16. Hall, C. B., C. E. Long, K. C. Schnabel, M. T. Caserta, K. M. McIntyre, M. A. Costanzo, A. Knott, S. Dewhurst, R. A. Insel, and L. G. Epstein. 1994. Human herpesvirus-6 infection in children. A prospective study of complications and reactivation. N. Engl. J. Med. 331:432-438[Abstract/Free Full Text].

17. Hata, A., T. Mukai, Y. Isegawa, and K. Yamanishi. 1996. Identification and analyses of glycoprotein B of human herpesvirus 7. Virus Res. 46:125-137[CrossRef][Medline].

18. Herold, B. C., S. I. Gerber, B. J. Belval, A. M. Siston, and N. Shulman. 1996. Differences in the susceptibility of herpes simplex virus types 1 and 2 to modified heparin compounds suggest serotype differences in viral entry. J. Virol. 70:3461-3469[Abstract].

19. Herold, B. C., S. I. Gerber, T. Polonsky, B. J. Belval, P. N. Shaklee, and K. Holme. 1995. Identification of structural features of heparin required for inhibition of herpes simplex virus type 1 binding. Virology 206:1108-16[CrossRef][Medline].

20. Herold, B. C., and P. G. Spear. 1994. Neomycin inhibits glycoprotein C (gC)-dependent binding of herpes simplex virus type 1 to cells and also inhibits postbinding events in entry. Virology 203:166-171[CrossRef][Medline].

21. Herold, B. C., D. WuDunn, N. Soltys, and P. G. Spear. 1991. Glycoprotein C of herpes simplex virus type 1 plays a principal role in the adsorption of virus to cells and in infectivity. J. Virol. 65:1090-1098[Abstract/Free Full Text].

22. Hidaka, Y., K. Okada, K. Kusuhara, C. Miyazaki, K. Tokugawa, and K. Ueda. 1994. Exanthem subitum and human herpesvirus 7 infection. Pediatr. Infect. Dis. J. 13:1010-1011[Medline].

23. Johnson, D. C., and M. W. Ligas. 1988. Herpes simplex viruses lacking glycoprotein D are unable to inhibit virus penetration: quantitative evidence for virus-specific cell surface receptors. J. Virol. 62:4605-4612[Abstract/Free Full Text].

24. Kari, B., and R. Gehrz. 1993. Structure, composition and heparin binding properties of a human cytomegalovirus glycoprotein complex designated gC-II. J. Gen. Virol. 74:255-64[Abstract/Free Full Text].

25. Kozak, M. 1987. An analysis of 5'-noncoding sequences from 699 vertebrate messenger RNAs. Nucleic Acids Res. 15:8125-8148[Abstract/Free Full Text].

26. Lusso, P., P. Secchiero, R. W. Crowley, A. Garzino-Demo, Z. N. Berneman, and R. C. Gallo. 1994. CD4 is a critical component of the receptor for human herpesvirus 7: interference with human immunodeficiency virus. Proc. Natl. Acad. Sci. USA 91:3872-3876[Abstract/Free Full Text].

27. Megaw, A. G., D. Rapaport, B. Avidor, N. Frenkel, and A. J. Davison. 1998. The DNA sequence of the RK strain of human herpesvirus 7. Virology 244:119-132[CrossRef][Medline].

28. Mukai, T., A. Hata, Y. Isegawa, and K. Yamanishi. 1997. Characterization of glycoprotein H and L of human herpesvirus 7. Microbiol. Immunol. 41:43-50[Medline].

29. Nicholas, J. 1996. Determination and analysis of the complete nucleotide sequence of human herpesvirus-7. J. Virol. 70:5975-5989[Abstract].

30. Pereira, L. 1994. Function of glycoprotein B homologues of the family herpesviridae. Infect. Agents Dis. 3:9-28[Medline].

31. Petrovskis, E. A., A. L. Meyer, and L. E. Post. 1988. Reduced yield of infectious pseudorabies virus and herpes simplex virus from cell lines producing viral glycoprotein gp50. J. Virol. 62:2196-2199[Abstract/Free Full Text].

32. Pfeiffer, B., Z. N. Berneman, F. Neipel, C. K. Chang, S. Tirwatnapong, and B. Chandran. 1993. Identification and mapping of the gene encoding the glycoprotein complex gp82-gp105 of human herpesvirus 6 and mapping of the neutralizing epitope recognized by monoclonal antibodies. J. Virol. 67:4611-4620[Abstract/Free Full Text].

33. Pfeiffer, B., B. Thomson, and B. Chandran. 1995. Identification and characterization of a cDNA derived from multiple splicing that encodes envelope glycoprotein gp105 of human herpesvirus 6. J. Virol. 69:3490-3500[Abstract].

34. Portolani, M., C. Cermelli, P. Mirandola, and D. Di Luca. 1995. Isolation of human herpesvirus 7 from an infant with febrile syndrome. J. Med. Virol. 45:282-283[Medline].

35. Pruksananonda, P., C. B. Hall, R. A. Insel, K. McIntyre, P. E. Pellett, C. E. Long, K. C. Schnabel, P. H. Pincus, F. R. Stamey, T. R. Dambaugh, and J. A. Stewart. 1992. Primary human herpesvirus 6 infection in young children. N. Engl. J. Med. 326:1445-1450[Abstract].

36. Roizman, B., and A. E. Sears. 1996. Herpes simplex viruses and their replication, p. 2231-2296. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed., vol. 2. Lippincott-Raven, Philadelphia, Pa.

37. Rostand, K. S., and J. D. Esko. 1997. Microbial adherence to and invasion through proteoglycans. Infect. Immun. 65:1-8[Medline].

38. Salahuddin, S. Z., D. V. Ablashi, P. D. Markham, S. F. Josephs, S. Sturzenegger, M. Kaplan, G. Halligan, P. Biberfeld, F. Wong-Staal, B. Kramarsky, and R. C. Gallo. 1986. Isolation of a new virus, HBLV, in patients with lymphoproliferative disorders. Science 234:596-601[Abstract/Free Full Text].

39.

1.	Baum, B. 1995. Salivary gland repair. Adv. Dental Res. 9:22[Medline].
2.	Berneman, Z. N., D. V. Ablashi, G. Li, M. Eger-Fletcher, M. S. Reitz, Jr., C. L. Hung, I. Brus, A. L. Komaroff, and R. C. Gallo. 1992. Human herpesvirus 7 is a T-lymphotropic virus and is related to, but significantly different from, human herpesvirus 6 and human cytomegalovirus. Proc. Natl. Acad. Sci. USA 89:10552-10556[Abstract/Free Full Text].
3.	Black, J. B., N. Inoue, K. Kite-Powell, S. Zaki, and P. E. Pellett. 1993. Frequent isolation of human herpesvirus 7 from saliva. Virus Res. 29:91-98[CrossRef][Medline].
4.	Black, J. B., T. F. Schwarz, J. L. Patton, K. Kite-Powell, P. E. Pellett, S. Wiersbitzky, R. Bruns, C. Muller, G. Jager, and J. A. Stewart. 1996. Evaluation of immunoassays for detection of antibodies to human herpesvirus 7. Clin. Diagn. Lab. Immunol. 3:79-83[Abstract].
5.	Caldwell, E. E., V. D. Nadkarni, J. R. Fromm, R. J. Linhardt, and J. M. Weiler. 1996. Importance of specific amino acids in protein binding sites for heparin and heparan sulfate. Int. J. Biochem. Cell Biol. 28:203-216[CrossRef][Medline].
6.	Campadelli-Fiume, G., M. Arsenakis, F. Farabegoli, and B. Roizman. 1988. Entry of herpes simplex virus 1 in BJ cells that constitutively express viral glycoprotein D is by endocytosis and results in degradation of the virus. J. Virol. 62:159-67[Abstract/Free Full Text].
7.	Cardin, A. D., and H. J. Weintraub. 1989. Molecular modeling of protein-glycosaminoglycan interactions. Arteriosclerosis 9:21-32[Abstract/Free Full Text].
8.	Devereux, J., P. Haeberli, and O. Smithies. 1984. A comprehensive set of sequence analysis programs for the VAX. Nucleic Acids Res. 12:387-395.
9.	Di Luca, D., P. Mirandola, T. Ravaioli, R. Dolcetti, A. Frigatti, P. Bovenzi, L. Sighinolfi, P. Monini, and E. Cassai. 1995. Human herpesviruses 6 and 7 in salivary glands and shedding in saliva of healthy and human immunodeficiency virus positive individuals. J. Med. Virol. 45:462-468[Medline].
10.	Flynn, S. J., and P. Ryan. 1996. The receptor-binding domain of pseudorabies virus glycoprotein gC is composed of multiple discrete units that are functionally redundant. J. Virol. 70:1355-1364[Abstract].
11.	Foa-Tomasi, L., E. Avitabile, L. Ke, and G. Campadelli-Fiume. 1994. Polyvalent and monoclonal antibodies identify major immunogenic proteins specific for human herpesvirus 7-infected cells and have weak cross-reactivity with human herpesvirus 6. J. Gen. Virol. 75:2719-2727[Abstract/Free Full Text].
12.	Frenkel, N., E. C. Schirmer, L. S. Wyatt, G. Katsafanas, E. Roffman, R. M. Danovich, and C. H. June. 1990. Isolation of a new herpesvirus from human CD4⁺ T cells. Proc. Natl. Acad. Sci. USA 87:748-752[Abstract/Free Full Text].
13.	Frenkel, N., and L. S. Wyatt. 1992. HHV-6 and HHV-7 as exogenous agents in human lymphocytes. Dev. Biol. Stand. 76:259-265[Medline].
14.	Fromm, J. R., R. E. Hileman, E. E. Caldwell, J. M. Weiler, and R. J. Linhardt. 1997. Pattern and spacing of basic amino acids in heparin binding sites. Arch. Biochem. Biophys. 343:92-100[CrossRef][Medline].
15.	Gompels, U. A., J. Nicholas, G. Lawrence, M. Jones, B. J. Thomson, M. E. Martin, S. Efstathiou, M. Craxton, and H. A. Macaulay. 1995. The DNA sequence of human herpesvirus-6: structure, coding content, and genome evolution. Virology 209:29-51[CrossRef][Medline].
16.	Hall, C. B., C. E. Long, K. C. Schnabel, M. T. Caserta, K. M. McIntyre, M. A. Costanzo, A. Knott, S. Dewhurst, R. A. Insel, and L. G. Epstein. 1994. Human herpesvirus-6 infection in children. A prospective study of complications and reactivation. N. Engl. J. Med. 331:432-438[Abstract/Free Full Text].
17.	Hata, A., T. Mukai, Y. Isegawa, and K. Yamanishi. 1996. Identification and analyses of glycoprotein B of human herpesvirus 7. Virus Res. 46:125-137[CrossRef][Medline].
18.	Herold, B. C., S. I. Gerber, B. J. Belval, A. M. Siston, and N. Shulman. 1996. Differences in the susceptibility of herpes simplex virus types 1 and 2 to modified heparin compounds suggest serotype differences in viral entry. J. Virol. 70:3461-3469[Abstract].
19.	Herold, B. C., S. I. Gerber, T. Polonsky, B. J. Belval, P. N. Shaklee, and K. Holme. 1995. Identification of structural features of heparin required for inhibition of herpes simplex virus type 1 binding. Virology 206:1108-16[CrossRef][Medline].
20.	Herold, B. C., and P. G. Spear. 1994. Neomycin inhibits glycoprotein C (gC)-dependent binding of herpes simplex virus type 1 to cells and also inhibits postbinding events in entry. Virology 203:166-171[CrossRef][Medline].
21.	Herold, B. C., D. WuDunn, N. Soltys, and P. G. Spear. 1991. Glycoprotein C of herpes simplex virus type 1 plays a principal role in the adsorption of virus to cells and in infectivity. J. Virol. 65:1090-1098[Abstract/Free Full Text].
22.	Hidaka, Y., K. Okada, K. Kusuhara, C. Miyazaki, K. Tokugawa, and K. Ueda. 1994. Exanthem subitum and human herpesvirus 7 infection. Pediatr. Infect. Dis. J. 13:1010-1011[Medline].
23.	Johnson, D. C., and M. W. Ligas. 1988. Herpes simplex viruses lacking glycoprotein D are unable to inhibit virus penetration: quantitative evidence for virus-specific cell surface receptors. J. Virol. 62:4605-4612[Abstract/Free Full Text].
24.	Kari, B., and R. Gehrz. 1993. Structure, composition and heparin binding properties of a human cytomegalovirus glycoprotein complex designated gC-II. J. Gen. Virol. 74:255-64[Abstract/Free Full Text].
25.	Kozak, M. 1987. An analysis of 5'-noncoding sequences from 699 vertebrate messenger RNAs. Nucleic Acids Res. 15:8125-8148[Abstract/Free Full Text].
26.	Lusso, P., P. Secchiero, R. W. Crowley, A. Garzino-Demo, Z. N. Berneman, and R. C. Gallo. 1994. CD4 is a critical component of the receptor for human herpesvirus 7: interference with human immunodeficiency virus. Proc. Natl. Acad. Sci. USA 91:3872-3876[Abstract/Free Full Text].
27.	Megaw, A. G., D. Rapaport, B. Avidor, N. Frenkel, and A. J. Davison. 1998. The DNA sequence of the RK strain of human herpesvirus 7. Virology 244:119-132[CrossRef][Medline].
28.	Mukai, T., A. Hata, Y. Isegawa, and K. Yamanishi. 1997. Characterization of glycoprotein H and L of human herpesvirus 7. Microbiol. Immunol. 41:43-50[Medline].
29.	Nicholas, J. 1996. Determination and analysis of the complete nucleotide sequence of human herpesvirus-7. J. Virol. 70:5975-5989[Abstract].
30.	Pereira, L. 1994. Function of glycoprotein B homologues of the family herpesviridae. Infect. Agents Dis. 3:9-28[Medline].
31.	Petrovskis, E. A., A. L. Meyer, and L. E. Post. 1988. Reduced yield of infectious pseudorabies virus and herpes simplex virus from cell lines producing viral glycoprotein gp50. J. Virol. 62:2196-2199[Abstract/Free Full Text].
32.	Pfeiffer, B., Z. N. Berneman, F. Neipel, C. K. Chang, S. Tirwatnapong, and B. Chandran. 1993. Identification and mapping of the gene encoding the glycoprotein complex gp82-gp105 of human herpesvirus 6 and mapping of the neutralizing epitope recognized by monoclonal antibodies. J. Virol. 67:4611-4620[Abstract/Free Full Text].
33.	Pfeiffer, B., B. Thomson, and B. Chandran. 1995. Identification and characterization of a cDNA derived from multiple splicing that encodes envelope glycoprotein gp105 of human herpesvirus 6. J. Virol. 69:3490-3500[Abstract].
34.	Portolani, M., C. Cermelli, P. Mirandola, and D. Di Luca. 1995. Isolation of human herpesvirus 7 from an infant with febrile syndrome. J. Med. Virol. 45:282-283[Medline].
35.	Pruksananonda, P., C. B. Hall, R. A. Insel, K. McIntyre, P. E. Pellett, C. E. Long, K. C. Schnabel, P. H. Pincus, F. R. Stamey, T. R. Dambaugh, and J. A. Stewart. 1992. Primary human herpesvirus 6 infection in young children. N. Engl. J. Med. 326:1445-1450[Abstract].
36.	Roizman, B., and A. E. Sears. 1996. Herpes simplex viruses and their replication, p. 2231-2296. In B. N. Fields, D. M. Knipe, and P. M. Howley (ed.), Fields virology, 3rd ed., vol. 2. Lippincott-Raven, Philadelphia, Pa.
37.	Rostand, K. S., and J. D. Esko. 1997. Microbial adherence to and invasion through proteoglycans. Infect. Immun. 65:1-8[Medline].
38.	Salahuddin, S. Z., D. V. Ablashi, P. D. Markham, S. F. Josephs, S. Sturzenegger, M. Kaplan, G. Halligan, P. Biberfeld, F. Wong-Staal, B. Kramarsky, and R. C. Gallo. 1986. Isolation of a new virus, HBLV, in patients with lymphoproliferative disorders. Science 234:596-601[Abstract/Free Full Text].
39.