The U69 Gene of Human Herpesvirus 6 Encodes a Protein Kinase Which Can Confer Ganciclovir Sensitivity to Baculoviruses

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Ansari, A.
	Articles by Emery, V. C.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Ansari, A.
	Articles by Emery, V. C.

Previous Article | Next Article

Journal of Virology, April 1999, p. 3284-3291, Vol. 73, No. 4
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

The U69 Gene of Human Herpesvirus 6 Encodes a Protein Kinase Which Can Confer Ganciclovir Sensitivity to Baculoviruses

Azeem Ansari and Vincent C. Emery^*

Department of Virology, Royal Free and University College Medical School, University College London, Royal Free Campus, Hampstead, London NW3 2PF, United Kingdom

Received 23 September 1998/Accepted 4 January 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The protein encoded by the U69 open reading frame (ORF) of human herpesvirus 6 (HHV-6) has been predicted to be a proteinkinase. To investigate its functional properties, we have expressedthe U69 ORFs from both HHV-6 variants, A and B, by using recombinantbaculoviruses (BV6AU69 and BV6BU69). Nickel agarose and antibodyaffinity chromatography was used to purify the proteins to homogeneityand when incubated with [ $gamma$ -³²P]ATP, both U69 proteins became phosphorylated on predominantlyserine residues. These data strongly suggest that U69 is a proteinkinase which autophosphorylates. The phosphorylation reactionwas optimal at physiological pH and low NaCl concentrations. Itrequired the presence of Mg²⁺ or Mn²⁺, and Mg²⁺ was able to support phosphorylation over a wider range of concentrationsthan Mn²⁺. Both ATP and GTP could donate phosphate in the protein kinaseassay and the former was more efficient. U69 was capable of phosphorylatinghistone and casein (serine/threonine kinase substrates) but notenolase (a tyrosine kinase substrate). For the autophosphorylationreaction, the Michaelis constants for ATP of baculovirus-expressedHHV-6A and HHV-6B U69 were calculated to be 44 and 11 µM, respectively.U69 is a homologue of the UL97 gene encoded by human cytomegaloviruswhich has been shown to phosphorylate the antiviral drug ganciclovir(GCV). We analyzed whether the U69 ORF alone was capable of conferringGCV sensitivity on baculoviruses BV6AU69 and BV6BU69. In plaquereduction experiments, these baculoviruses displayed a GCV-sensitivephenotype compared to a control baculovirus (BVLacZ). The 50%inhibitory concentrations (IC₅₀) of BV6AU69 and BV6BU69 were calculatedto be 0.35 and 0.26 mM, respectively, whereas the control baculovirushad an IC₅₀ of >1.4 mM. This shows that the U69 gene product isthe only one required to confer GCV sensitivity onbaculovirus.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Human herpesvirus 6 (HHV-6) was first isolated from the peripheral blood of patients with lymphoproliferative disorders (1,44). The DNA sequence of HHV-6 (strain U1102) has been published(20), and analysis has revealed that the overall arrangementof genes is similar to that of human cytomegalovirus (HCMV), with66% of the DNA sequence showing homology (30); therefore, HHV-6has been classified as a betaherpesvirus. As with all other humanherpesviruses, primary infection is followed by lifelong persistencein the host. HHV-6 is widespread throughout the world's population,with about 90% seroconverting within the first 2 years of life(40, 45, 52).

HHV-6 can be further subdivided into two distinct groups, variants A and B (17), and in infants, primary HHV-6B infectioncauses febrile illness including exanthem subitum (41, 51).The epidemiology and clinical consequences of HHV-6A infectionsare not as fully defined; however, primary HHV-6A infection hasbeen reported in one case of exanthem subitum (25). HHV-6 infectionshave also been associated with encephalitis (4), hepatitis(3), multiple sclerosis, chronic fatigue syndrome, and somelymphomas, although a formal causal association has not been proven(5, 7, 31, 48). In individuals who are immunosuppressedby drugs, such as transplant patients, or individuals infectedwith human immunodeficiency virus, HHV-6 is emerging as an importantpathogen. In bone marrow transplant recipients, both HHV-6A andHHV-6B have been associated with marrow suppression, pneumonitis,graft-versus-host disease, and encephalitis (9, 10, 18,24, 28, 29, 43, 53). In individuals infected with humanimmunodeficiency virus, HHV-6 has been implicated as being a cofactorin disease progression (34).

Ganciclovir (GCV), a nucleoside analogue, is the first-choice antiviral agent used to treat HCMV infections. However, no drugshave been tested in a controlled manner to determine efficacyin treating HHV-6 infections. In vitro, the overall antiviralsusceptibility of HHV-6 to a range of antiviral drugs is similarto that of HCMV (2, 8), and an interesting feature of onestudy is that GCV was found to be more effective against HHV-6Athan against HHV-6B (50). If this result is confirmed, thenit may have important implications for the treatment of HHV-6infections.

The mechanism of action of GCV depends on the formation of the triphosphate form via sequential phosphorylation at the 5'-hydroxylposition. The UL97 protein kinase encoded by HCMV is responsiblefor the monophosphorylation of GCV, and resistance to the drughas been mapped to this gene (12, 22, 32, 33, 35, 47,49). Sequence analysis revealed that HHV-6 codes for a homologueof UL97, the U69 gene, which has been implicated as a functionalhomologue (32, 11, 16). The U69 gene shows homology to proteinkinases and belongs to a family of genes encoded by all herpesviruses,many of which have been shown to catalyze the transfer of phosphatesonto target molecules or proteins (11, 13, 14, 16, 23,26, 37-39, 42). The precise biological function performed bythe herpesvirus kinases in the virus life cycle remains to beelucidated; however, their ability to phosphorylate proteins,many of which may have important regulatory roles in virus replication,makes them potential targets for antiviral intervention. Therefore,further information about this class of protein may facilitatethe discovery of new and more effective antiherpesviruscompounds.

In order to characterize the U69 genes of both HHV-6A and HHV-6B, we have expressed them in heterologous expression systemsand purified them to homogeneity by using polyclonal monospecificantisera. The data presented here demonstrate that the U69 genecan confer GCV sensitivity on baculovirus, is a protein kinasethat autophosphorylates predominately on serine residues, andcan catalyze the phosphorylation of exogenous substrates. In addition,we present evidence that the U69 proteins of HHV-6A and HHV-6Bhave differential protein kinaseactivities.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and viruses. Spodoptera frugiperda 21 (Sf21) cells (Invitrogen) were maintained in TC100 medium (Life Technologies) supplemented with 10%fetal bovine serum, 50 IU of penicillin per ml, and 50 µg of streptomycinper ml. Wild-type linearized Autographa californica multiple nuclearpolyhedrosis virus (AcMNPV; Invitrogen) was used to constructthe recombinant baculoviruses. HHV-6A (AJ) and HHV-6B (Z29) werepropagated in the J-Jhan and Molt-3 continuous T-cell lines, respectively.Both cell lines were maintained in RPMI medium (Life Technologies)supplemented with 10% fetal bovine serum, 2 mM L-glutamine, 100IU of penicillin per ml, and 100 µg of streptomycin per ml in5% CO₂.

Cloning and sequencing of the HHV-6A and HHV-6B U69 ORFs. Total DNA was extracted from HHV-6A- and HHV-6B-infected cells in culture by using the Puregene DNA isolation kit and usedas a PCR template to generate full-length U69 open reading frames(ORFs). The primers (IP1-BamHI, dGATCGATGGATCCGAATAATTATGGACAACGGTGTGGA;IP2-HindIII, dTGCAGTCAAGCTTTCCATTACTATATCACATATGAAAG) were designedsuch that the PCR would generate an amplicon with a BamHI siteat the 5' position and a HindIII site at the 3' position. To minimizeTaq-generated errors, Bio-X-Act (Bioline) proofreading enzymewas used in the PCR as recommended by the manufacturer. The PCRgenerated a single DNA fragment approximately 1.7 kb long whichwas purified by standard phenol chloroform extraction and ethanolprecipitation. The amplicons were then restricted with BamHI andHindIII and cloned into appropriately digested baculovirus transfervector pBluBacHis (Invitrogen) downstream of a 4-kDa tag, generatingplasmids pblu6AU69 and pblu6BU69 (Fig. 1). The N-terminal tagconsists of six tandem histidine residues and an antibody recognitionsite (RGSHis). The clones were identified and distinguished byrestriction enzyme analysis. To confirm that the U69 ORFs hadbeen inserted downstream and in frame with respect to the fusion,the plasmid clones were DNA sequenced by the Sequenase version2.0 protocol (United States Biochemical). In order to allow forexpression in Escherichia coli, pblu6AU69 and pblu6BU69 were restrictedwith BamHI and HindIII and the DNA fragments were separated byagarose gel electrophoresis. The U69 ORFs were excised from thegel, purified via the Gene Clean method (Bio 101), and clonedinto bacterial expression vector pTrcHisC (Invitrogen), producingthe plasmids pTrc6AU69 and pTrc6BU69. Proteins expressed fromthese E. coli-based vectors are N-terminal fusions identical tothe baculovirus transfer vectors described above.

View larger version (17K):
[in this window]
[in a new window]

FIG. 1. Cloning of the HHV-6A and HHV-6B U69 proteins. (A) Schematic organization of the HHV-6 genome with terminal direct repeats (

) and a unique region (U). The scale is marked in kilobase pairs. (B) PCR primers IP1-BamHI and IP2-HindIII generated HHV-6A and HHV-6B U69 amplicons which had restriction endonuclease recognition sites at either end to allow subsequent cloning of the amplicons into appropriately digested baculovirus transfer vector pBluBacHis. (C) Recombinant baculoviruses (BV6AU69 and BV6BU69) were constructed containing the HHV-6 U69 gene driven by the polyhedrin promoter ( &cjs3605;

). The U69 protein was expressed as an N-terminal antibody epitope (RGSHis) and polyhistidine [(His)₅] fusion.

Construction of recombinant baculoviruses. From each of the transfer vectors (pblu6AU69 and pblu6BU69), a recombinant baculovirus was constructed by cotransfecting themindividually with linear, wild-type AcMNPV DNA using Insectin-Plusliposomes (Invitrogen). By standard methodologies, recombinantbaculoviruses BV6AU69 and BV6BU69 were isolated by two roundsof plaque purification and expanded into high-titer virus stocks(27). The insertion of the U69 gene into the baculovirus genomeand the absence of contaminating wild-type AcMNPV were confirmedbyPCR.

Preparation of U69-specific IgG. A 5-liter Luria-Bertani (LB) broth (Sigma) culture of E. coli BL21 (Novagene) harboring pTrc6AU69 was grown to an A₆₀₀ of0.6, and expression of the recombinant protein was induced byaddition of isopropyl- $beta$ -D-thiogalactopyranoside (IPTG) to a finalconcentration of 0.5 mM. Cells were harvested by centrifugationafter a 6-h postinduction period and resuspended in ice-cold lysisbuffer A (50 mM NaH₂PO₄ [pH 8.0], 300 mM NaCl, 10 mM $beta$ -mercaptoethanol,1 mM pefabloc [Boehringer Mannheim], 10 mg of lysosome per ml,1% Triton X-100). The bacteria were incubated on ice for 1 h andsonicated (3 × 15 s), and soluble material was removed by ultracentrifugationat 30,000 × g. The E. coli-expressed U69 protein cosedimentedwith the insoluble fraction, which was then resuspended in ice-coldbuffer B (50 mM NaH₂PO₄ [pH 8.0], 300 mM NaCl, 10 mM $beta$ -mercaptoethanol,1 mM pefabloc [Boehringer Mannheim], 1.5% sarkosyl) and sonicatedas described above. The supernatant was clarified by centrifugationat 30,000 × g and loaded onto a nickel-nitrilotriacetic acid (Ni²⁺-NTA [Qiagen]) column. The column was washed with excess ice-coldbuffer B containing 10 mM imadizole, and bound protein was elutedwith ice-cold buffer B containing 500 mM imadizole. This methodresulted in a single species of protein upon analysis of the eluateby sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)and Coomassie brilliant blue staining. The sheep antisera wereprepared by the Scottish Antibody Production Unit. The initialimmunization used 250 µg of antigen in Freund's complete adjuvant.The animal was subsequently boosted a further three times withthe same amount of antigen at 28-day intervals, and the finalantiserum was collected on day 112. The serum was found to containa low level of antibodies reactive against bacterial proteins,which were subsequently removed by incubating the antisera withimmobilized protein extracts from E. coli cells harboring pTrcHis.The immunoglobulin G (IgG) component of the antisera was capturedfrom the serum by using a protein G column (Pharmacia), eluted,and immobilized on CNBr-activated Sepharose 4B (Pharmacia) inaccordance with the manufacturer'smethods.

Western analysis of protein expression. Proteins were separated by SDS-PAGE and electrophoretically transferred onto a polyvinylidene difluoride (PVDF; Bio-Rad) membraneby using a semidry blotter (Pharmacia Biotech). The membrane wasincubated for 1 h at room temperature in blocking buffer consistingof 3% bovine serum albumin (Sigma) in TBS (10 mM Tris-HCl [pH7.5], 150 mM NaCl) and then washed with 0.05% Tween 20-0.1% TritonX-100 in TBS (wash buffer). The membrane was then incubated withthe RGSHis (Qiagen) murine primary antibody or with U69-specificantisera for 1 h at room temperature, diluted to 1:1,000 or 1:10,000,respectively, in blocking buffer, and then further washed. Goatanti-mouse IgG (Bio-Rad) or goat anti-sheep IgG (Sigma) conjugatedto alkaline phosphatase, diluted to 1:6,000 in blocking buffer,was used as the secondary antibody and incubated with the membranefor 1 h at room temperature. The membrane was further washed,and immunoreactive bands were visualized by incubation of themembrane in a staining solution consisting of one tablet of 5-bromo-4-chloro-3-indolylphosphate-nitrobluetetrazolium chloride (Sigma) dissolved in 10 ml of distilled H₂O.

Purification of baculovirus-expressed U69 protein. Sf21 cells (6 × 10⁶) were infected with BV6AU69 or BV6BU69 at a multiplicity of infection (MOI) of 5 and incubated at 28°C.Infected cells were harvested at 72 h postinfection, and the culturemedium was removed by centrifugation at 1,000 × g. The cell pelletwas washed twice with 10 ml of phosphate-buffered saline and resuspendedin 0.5 ml of ice-cold buffer C (50 mM Tris-HCl [pH 7.6], 100 mMNaCl, 5 mM MgCl₂, 0.1% Nonidet P-40, 10% glycerol, 10 µg of apoprotininper ml, 10 µg of leupeptin per ml, 1 mM pefabloc). The cells weresonicated on ice for 10 s three times with 30 s of cooling inbetween. All subsequent procedures were carried out at 4°C. Insolublematerial was removed by centrifugation at 13,000 × g in a desktopmicrocentrifuge for 10 min, and 50 µl of a 50% slurry of Ni²⁺-NTA pre-equilibrated with buffer C was added to the soluble extractand allowed to bind for 1 h with constant gentle agitation. TheNi²⁺-NTA was then pelleted in a benchtop microcentrifuge for 12 sat 13,000 × g and washed three times with excess buffer C containing10 mM imadizole. Bound proteins were eluted by incubating theNi²⁺-NTA in 100 µl of buffer C containing 500 mM imadizole. The enzymewas further purified by mixing the eluate with 100 µl (50% slurrypre-equilibrated with buffer C) of immobilized U69-specific IgGand allowed to bind for 1 h. The Sepharose beads were then washedthree times with buffer C containing 0.5 M NaCl and twice withbuffer C. To measure the amount of specific U69 complexed withthe antibody, equal volumes of immunoprecipitate were subjectedto SDS-PAGE alongside standards of known amounts of bovine serumalbumin. The gel was silver stained and scanned by using a Bio-RadFluoroimager, the densities of the bands corresponding to theprotein standards were measured by using Multianalyst software,and a standard curve was generated from this. Because the densityof the band corresponding to the U69 protein was known, the amountof U69 protein that complexed with the antibody could be extrapolatedfrom the standardcurve.

Protein kinase assays. Protein samples were added to 20 µl of kinase buffer (50 mM Tris-HCl [pH 9.0], 1 M NaCl, 10 mM MgCl₂, 2 mM dithiothreitol,5 µM ATP, 5 µCi of [ $gamma$ -³²P]ATP at >5,000 Ci/mmol [Amersham]) and incubated for 30 min,unless stated otherwise, with or without 1 mg of exogenous substrateper ml at 37°C. The reaction was terminated by the addition of20 µl of 2 × SDS sample buffer (125 mM Tris-HCl [pH 8.0], 2.0%SDS, 10% sucrose, 0.01% bromophenol blue), and the mixture wasboiled for 3 min. The reaction mixture was then subjected to SDS-PAGE,after which the gels were dried and exposed to Hyperfilm (Amersham).To quantify the amount of label incorporated, autoradiographswere digitized by using a Bio-Rad Fluoroimager, and the densitiesof appropriate bands were measured by using Multianalyst software(Bio-Rad). The Michaelis constant (K_m) for ATP was calculatedby standard Lineweaver-Burke analysis. Briefly, 2-min proteinkinase assays were performed in the presence of various totalATP concentrations. The reactions were terminated, and the reactionmixtures were separated by SDS-PAGE. The gel was exposed to film,and the amount of radiolabel incorporated for each ATP concentrationwas measured by densitometry. A Lineweaver-Burke graph of theinverse of the amount of radiolabel incorporated was plotted againstthe inverse of the corresponding ATP concentration, and the extrapolatedintercept on the x axis ( $-$ 1/K_m) determined the K_mvalue.

Phosphoamino acid analysis. The recombinant protein was partially purified, and 100 ng of protein was phosphorylated as described above. The reactionmixture was subjected to SDS-PAGE and electrophoretically transferredonto PVDF. The membrane was wrapped in Saran film (to preventdrying), and phosphorylated U69 protein was located by exposingthe membrane to X-ray film. The corresponding band was excisedfrom the membrane, and bound protein was hydrolyzed by heatingat 110°C in the presence of 6 M HCl for 60 min. The hydrolysatewas transferred to a fresh microcentrifuge tube and concentratedin a Speedvac evaporator. After the liquid had evaporated, thedessicate was resuspended in 6 µl of water and vortexed vigorouslyfor 5 min. Half of the sample was spotted onto a cellulose thin-layerchromatographic plate in 0.5-µl aliquots, which were allowed todry between loadings. Samples (0.3 ng each) of phosphoserine,phosphotyrosine, and phosphothreonine (Sigma) were also spottedas standards. The plate was subjected to two-dimensional electrophoresisat 1.5 kV for 20 min in pH 1.9 (88% formic acid-acetic acid-water,25:78:897) electrophoresis buffer in the first dimension and inpH 3.5 buffer (acetic acid-pyridine-100 mM EDTA-water, 50:5:5:940)for 20 min at 1.3 kV in the second dimension. The plate was developedwith 0.2% ninhydrin inethanol.

Plaque reduction assay. To test whether the U69 protein can confer GCV sensitivity on AcMNPV, plaque reduction experiments were performed as follows.Sf21 cells were infected at an MOI of 0.3. After an absorptionperiod of 1 h, the inoculum was removed and replaced with culturemedium containing GCV (concentrations between 0 and 1.4 mM). Afterincubation at 28°C for 72 h, the culture medium was harvestedand the virus was titrated by plaque assay. As a control, BVLacZ,which is a baculovirus containing the lacZ gene, was used. Thiswas considered an appropriate control because BV6AU69 and BV6BU69were constructed such that they also express $beta$ -galactosidase.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Recombinant-baculovirus expression of U69. In order to produce recombinant U69 protein, the gene was cloned into the pBluBacHis baculovirus transfer vector and recombinantbaculoviruses BV6AU69 and BV6BU69 were generated. ORFs clonedinto the above baculovirus transfer vector are fused at the Nterminus to a 4-kDa tag consisting of five tandem histidine residuesand an antibody recognition site. In initial experiments, therewas no antiserum available for U69 therefore expressed U69 wasdetected via RGSHis (Qiagen), which is an antibody directed tothe N-terminal fusion. Although the U69 gene was placed underthe control of the strong polyhedrin promoter, we found that U69was expressed relatively poorly, even under optimized conditions(MOI of 5 and harvesting at 72 h postinfection [p.i.]). Nevertheless,under these conditions, a novel ~67-kDa protein accumulated thathad polyhedrin promoter kinetics and reacted with the anti-RGSHisantibody. This protein was not present in either uninfected orBVLacZ (baculovirus expressing $beta$ -galactosidase)-infected cells(Fig. 2A). Despite the use of a number of insect cell lines andconditions, U69 expression could not be enhanced.

View larger version (49K):
[in this window]
[in a new window]

FIG. 2. Detection and phosphorylation of baculovirus-expressed U69. Insect cells were infected with recombinant baculovirus BV6AU69, BV6BU69, or BVLacZ and harvested at 24, 48, 60, and 72 h p.i. Protein extracts were prepared, incubated in a standard protein kinase assay (see Materials and Methods), and subjected to SDS-PAGE. The gels were then either analyzed by Western blotting (A) or exposed to autoradiography (B). The major phosphorylated species accumulated with polyhedrin promoter kinetics and comigrated with recombinant U69 as detected by Western blotting. The images shown here and in other figures are continuous two-tone images obtaining by scanning with a UMAX Astra 600S and Adobe Photoshop 4.0.

Protein kinase activity of U69. To investigate whether HHV-6 U69 could catalyze the transfer of radiolabelled phosphates from ATP, BV6AU69- and BV6BU69-infectedSf21 cells were harvested at 24, 48, 60, and 72 h p.i. and U69was partially purified. The protein preparations were subjectedto a protein kinase assay containing [ $gamma$ -³²P]ATP, followed by SDS-PAGE and autoradiography. A 67-kDa proteinwas found to be the major labelled species, which accumulatedwith polyhedrin promoter kinetics (Fig. 2B). The phosphorylatedspecies comigrated with U69 detected by Western blotting (Fig.2A), and no labelled species was apparent at this molecular masswhen protein extracts from BVLacZ- and mock-infected cells weresimilarly assayed (Fig. 2B), indicating that the U69 protein wasbeingphosphorylated.

To eliminate the possibility of the 4-kDa tag participating in the phosphorylation reaction, we similarly analyzed chloroamphenicolacetyltransferase (26 kDa) expressed by baculovirus (BV26kDa)as an identical fusion. A crude extract containing this proteinwas either used directly in a protein kinase assay or mixed witha partially purified sample of recombinant U69 and coincubatedin a protein kinase assay. Neither situation resulted in a labelledproduct of 30 kDa (data notshown).

Transfer of GCV susceptibility to baculovirus. To test whether introduction of HHV-6 U69 could confer GCV susceptibility on baculovirus, BV6AU69, BV6BU69, and BVLacZ (control)were cultured with increasing amounts of GCV. In preliminary experiments,concentrations of GCV above 2.0 mM were found to be cytotoxic(data not shown). Therefore, GCV concentrations between 0 and1.4 mM were used. The amount of virus replication was measuredby plaque assay after a 72-h incubation period, and titers wereplotted against GCV concentrations as percentages of the amountof virus produced in the absence of GCV. The data shown in Fig.3 illustrate that baculoviruses expressing HHV-6 U69 were moresensitive to GCV growth inhibition than was the control baculovirus.The 50% inhibitory concentrations (IC₅₀s) for BV6AU69 and BV6BU69were calculated to be 0.35 and 0.26 mM, respectively, whereasthe IC₅₀ of the control virus was estimated to be 2.2 mM by extrapolation.

View larger version (16K):
[in this window]
[in a new window]

FIG. 3. Baculovirus plaque reduction assays. Baculoviruses expressing the U69 ORFs of HHV-6A and HHV-6B (BV6AU69,

; BV6BU69,

) were individually cultured in increasing concentrations of GCV (0 to 1.4 mM), and the effect of the drug on virus replication was measured by plaque assay. The inhibitory effect of GCV was greater for the U69-expressing baculoviruses than for the control (BVlacZ, $black-triangle$ ). A slight reduction in plaque formation was observed for BvlacZ; however, this was at GCV concentrations near the cytotoxic concentration. The IC₅₀s were calculated to be 0.35 and 0.26 mM for BV6AU69 and BV6BU69, respectively. The IC₅₀ for the control virus could not be determined within this data set. The values shown are means of three independent experiments, each performed in duplicate.

Purification of U69. Although we increased the specific activity of U69 in a partially purified protein preparation compared to the specific activityof U69 in a crude extract (data not shown), we were unable topurify it further by Ni²⁺-NTA chromatography. Consequently, we expressed HHV-6 U69 in E.coli by using the pTrcHisC vector and found that U69 was expressedalmost exclusively as insoluble inclusion bodies. Although largeamounts of U69 were purified from this system, the enzyme wasnot active in the protein kinase assay and did not phosphorylateGCV in vitro (data not shown). However, the protein was used toimmunize sheep and produce antisera which could recognize thebaculovirus-expressed protein. The IgG component from the antiserawas immobilized on CNBr-activated Sepharose 4B and used to affinitypurify baculovirus-expressed U69 from partially purified preparations.This approach (using first Ni²⁺-NTA and then immunoaffinity chromatography) allowed us to producehighly purified baculovirus-expressed U69 as demonstrated by silverstaining (Fig. 4).

View larger version (73K):
[in this window]
[in a new window]

FIG. 4. Purification of BV6AU69- and BV6BU69-expressed U69. Aliquots of protein samples were taken from each step of the purification procedure and analyzed by SDS-PAGE followed by silver staining. Lanes 1 and 5 represent crude lysates of insect cells infected with BV6AU69 or BV6BU69, respectively. Eluates of the Ni²⁺-NTA affinity purification step (lanes 2 and 6) were then immobilized by immunoaffinity chromatography, and samples were loaded on lanes 3 and 7. Lanes 4 and 8 represent aliquots of immobilized IgG. The molecular sizes of the protein markers (lane M) are indicated on the left.

To test for a difference in phosphotransferase activity between the HHV-6A and HHV-6B U69 proteins, equal amounts of specificU69 (10 ng) were subjected to a protein kinase assay and phosphorylationwas detected by autoradiography (Fig. 5). This analysis revealedthat (i) the homogeneous U69 protein product incorporated radiolabelledphosphates, (ii) the HHV-6A and HHV-6B U69 proteins had a subtledifference in electrophoretic mobility, and (iii) the proteinband corresponding to HHV-6B U69 appeared to be more dense thanthe band corresponding to HHV-6A U69. Enzyme kinetic analysisof these proteins with respect to ATP revealed that HHV-6B U69had a higher affinity for ATP than did U69 of HHV-6A (K_ms, 11µM for HHV-6B U69 and 44 µM for HHV-6A U69).

View larger version (57K):
[in this window]
[in a new window]

FIG. 5. Phosphorylation of purified recombinant U69. Equal amounts of U69, purified from BV6AU69- or BV6BU69-infected insect cells, were incubated with [ $gamma$ -³²P]ATP in a protein kinase assay and subjected to SDS-PAGE (lanes 2 and 3, respectively). The gel was dried and exposed to film. The resulting autoradiograph is shown. Lane 4 is immobilized U69-specific IgG used for immunoprecipitation of BVLacZ-infected insect cells and subjected to a protein kinase assay as described above. The molecular sizes of the protein markers (lane M) are indicated on the left.

As a final test to determine if U69 was being phosphorylated by a baculovirus or insect cell protein kinase, purified U69was inactivated by exposure to low pH and coincubated in a standardprotein kinase assay with protein preparations from uninfectedor BV26kDa-infected cells. Neither situation resulted in a phosphorylatedproduct with a molecular weight corresponding to that of U69 (datanotshown).

Phosphoamino acid analysis. From sequence analysis of the U69 ORF and protein kinases, we have located the catalytic domains of U69 (data not shown).Of interest are domains VI (D₃₁₃ISPMN) and VIII (F₃₇₃NPGFRPL),which resemble the consensus sequence of a protein kinase thathas specificity for serines and threonines more closely ratherthan a protein kinase that has specificity for tyrosine residues(21). To determine U69 hydroxyamino acid specificity experimentally,partially purified U69 was phosphorylated in a kinase assay andsubjected to SDS-PAGE. The proteins were transferred onto a PVDFmembrane, and the band corresponding to U69 was excised and subjectedto phosphoamino acid analysis. The results suggested that theHHV-6A and HHV-6B U69 proteins are predominantly phosphorylatedon serine residues with a smaller degree of phosphorylation onthreonine residues (Fig. 6). No labelled species correspondingto phosphotyrosine was observed.

View larger version (77K):
[in this window]
[in a new window]

FIG. 6. Phosphoamino acid analysis of recombinant U69. U69 was partially purified with Ni²⁺-NTA and phosphorylated in vitro in the presence of [ $gamma$ -³²P]ATP. The proteins were separated by SDS-PAGE and transferred electrophoretically onto a PVDF membrane, and the band corresponding to phosphorylated U69 was excised and acid hydrolyzed. The hydrolysate was mixed with unlabelled phosphoamino acids, phosphoserine (P-SER), phosphothreonine (P-THR), and phosphotyrosine (P-TYR) and subjected to two-dimensional electrophoretic thin-layer chromatography. The unlabelled phosphoamino acids were visualized with ninhydrin, and the autoradiograph of the thin-layer chromatography plate for the phosphoaminoacid analysis of HHV-6A U69 is shown. Phosphoamino acid analysis of HHV-6B U69 revealed a similar autoradiograph. The labelled phosphoamino acids comigrated with P-SER and P-THR, and the migration of P-TYR is indicated by the dotted circle.

Biochemical analysis of autophosphorylation. The velocity of the autophosphorylation reaction with respect to time, by using first ATP as the phosphate donor and thenGTP, was investigated. Our results indicate that U69 could useboth nucleoside triphosphates as the phosphate donor, althoughATP was favored (Fig. 7A and B). The autophosphorylation was foundto be linear for approximately 15 min and reached a maximum afterapproximately 40 min. The subsequent biochemical analysis (withrespect to salt dependence, divalent cation specificity and concentration,and pH) were therefore performed by using 2-min reactions in orderto measure initial rates. Phosphorylation was maximal at physiologicalpH (7 to 7.5) (Fig. 8A) and tolerated a wide range of Mg²⁺ concentrations (0.2 to 100 mM were tested) with 60 to 80% ofthe activity still remaining at 100 mM (Fig. 8B). Mn²⁺ could substitute as a divalent cation (Fig. 8C) with a more restrictedrange (0.2 to 10 mM) and an optimum concentration of 2 mM. Ca²⁺ concentrations between 1 and 10 mM did not support phosphorylation.The optimum NaCl concentration required was approximately 0.5M (Fig. 8D), with 50% activity still remaining at 1.5 M. The HHV-6Aand HHV-6B U69 proteins had similar biochemical characteristics.

View larger version (27K):
[in this window]
[in a new window]

FIG. 7. Velocity of autophosphorylation of recombinant HHV-6A (A) and HHV-6B (B) U69 with respect to time. Protein kinase assays were performed for the times indicated by using either ATP (

) or GTP ( $open circle$ ) as the radiolabelled phosphate donor. The reaction was terminated and subjected to SDS-PAGE. The amount of radiolabelled phosphate incorporation was measured by densitometry of the autoradiographs.

View larger version (26K):
[in this window]
[in a new window]

FIG. 8. Biochemical characteristics of HHV-6A (

) and HHV-6B ( $open circle$ ) U69. Baculovirus-expressed U69 was subjected to a standard protein kinase assay using radiolabelled ATP as the phosphate donor, except that the pH (A), divalent cation concentration (B and C), and NaCl concentration (D) were varied as indicated. In order to measure initial rates, 2-min reactions were performed. Autophosphorylation was measured for each condition by densitometry.

Phosphorylation of exogenous substrates. To test the ability of the protein kinase associated with HHV-6 U69 to catalyze the phosphorylation of exogenous substrates,histones, casein (serine/threonine protein kinase substrates),or enolase (a tyrosine protein kinase substrate) was mixed individuallywith purified U69 and incubated with [ $gamma$ -³²P]ATP in a protein kinase assay. The fact that only histones andcasein were phosphorylated (Fig. 9) is further evidence that U69is a protein kinase that has specificity for serine and threonineresidues.

View larger version (74K):
[in this window]
[in a new window]

FIG. 9. Phosphorylation of exogenous substrates. Purified U69 was coincubated in a protein kinase assay with exogenous proteins. The reaction was terminated, samples were subjected to SDS-PAGE, and the gel was exposed to film. The autoradiograph shows purified U69 from BV6AU69-infected insect cells incubated either alone (lane 2) or with histone casein or enolase (lanes 3 to 5) and purified U69 from BV6BU69-infected insect cells incubated either alone (lane 6) or with the exogenous substrates indicated (lanes 7 to 9). The positions and molecular sizes of marker proteins (lane M) are shown on the left side, and the migration of the exogenous substrates is shown on the right side. Lanes 10 to 12 are the exogenous substrates incubated in the absence of U69 in a standard protein kinase assay.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

It has been known for a number of years that HCMV infection in individuals undergoing organ transplantation is associatedwith significant morbidity, and there is increasing evidence thatHHV-6 is also as an important pathogen in such individuals (48).HCMV infections are usually treated with GCV, which has been shownto cause a rapid reduction in viremia (6). It has been found(2, 8, 50), albeit in vitro, that HHV-6 replication canalso be controlled with GCV; however, the precise molecular mechanismwhich governs the susceptibility of HHV-6 to the drug has yetto be investigated. The UL97 protein of HCMV has been shown todirect the phosphorylation of GCV in HCMV-infected cells. We describehere for the first time the molecular characterization of theprotein encoded by the U69 ORFs of both HHV-6A and HHV-6B, sequencehomologues of the HCMV UL97 ORF. Our results indicate that U69is a protein kinase that autophosphorylates on serine or threonineresidues and can also confer GCV sensitivity onbaculovirus.

When partially purified preparations of baculovirus-expressed U69 were incubated with [ $gamma$ -³²P]ATP, a radiolabelled species was apparent which comigrated withU69 detected by Western analysis, indicating that U69 may haveautophosphorylating properties. It was possible that this activitywas either inherent within the U69 protein itself or it was asubstrate for a cellular or baculovirus-encoded protein kinase.We favored the former for the following reasons. U69 is a sequencehomologue of a family of proteins encoded by all known herpesviruses,many of which have been shown to have phosphotransferase activity.For example, herpes simplex virus type 2 UL13 has been purifiedand shown to phosphorylate casein (15), and herpes simplex virustype 1 UL13 has been reported by several investigators to exhibitsimilar properties (14, 26, 42). HCMV UL97 and pseudorabiesvirus UL13 have been expressed in heterologous expression systems,and both have been shown to catalyze autophosphorylation in anin vitro kinase assay (16, 22). Although the varicella-zostervirus ORF 47 showed no phosphotransferase activity when producedin a heterologous expression system, it has been reported to autophosphorylatewhen immunoprecipitated from varicella-zoster virus-infected cells(37, 38). Cellular kinases, with the exception of casein kinase,are specific in the type of nucleotide triphosphate they utilizeto catalyze a phosphotransferase reaction. The herpesvirus kinasesstudied to date, like casein kinase, are unique in that they canutilize both ATP and GTP as a phosphate donor, and our data showthat U69 can also utilize both as phosphate donors. Nevertheless,it remains that U69 was serving as a substrate for phosphorylationby a cellular or baculovirus-encoded protein kinase. Subsequently,to investigate whether U69 could incorporate radiolabelled phosphatesin the absence of contaminating proteins, we highly purified U69and found that the phosphotransferase activity remained. Albeitunlikely, it may be possible that a contaminating kinase was copurifiedwith preparations of U69. To eliminate this possibility, purifiedU69 was inactivated and used as a substrate for phosphorylationby cellular or baculovirus-encoded proteins, and neither situationresulted in the phosphorylation of U69. Since protein kinasesrecognize a linear sequence as the target for phosphorylationand synthetic peptides are often used as substrates in experimentalprocedures, it follows that if the phosphorylation of U69 wasbeing carried out by a copurified kinase, then radiolabellingof U69 would be expected, irrespective of the physical state ofU69. Taken together, these data show that U69 is a protein kinasethat autophosphorylates and is a member of the family of kinasesencoded by all knownherpesviruses.

Despite the fact that they are members of the same family, there were significant differences in the biochemical propertiesof U69 and those reported for UL97 (22). Firstly, we found theU69 had a preference for low NaCl concentration (0.5 M), whereasthe HCMV UL97 has optimal activity at 1.5 M NaCl. Secondly, maximalU69 activity was observed at physiological pH, contrasting withHCMV UL97, which has a pH optimum of 9.5. The only biochemicalcharacteristic shared by U69 and UL97 was that both magnesiumand manganese could support phosphorylation. A possible explanationfor these apparent differences is that the proteins may play differentroles in the viral life cycle, including distinct viral or cellularsubstrates.

The majority of protein kinases can be classified into two categories, depending on their hydroxyamino acid specificity: (i)kinases that generate phosphate monoesters utilizing protein alcoholgroups (on serine or threonine) and (ii) ones that utilize proteinphenolic groups (on tyrosine) as phosphate acceptors. By analyzingthe sequences of subdomains VI and VIII, we were able to predictthe hydroxyamino acid specificity of U69 to be serine and threonine.We have confirmed this experimentally and shown that the majorityof the autophosphorylation occurs at serine residues, with threonineresidues being phosphorylated to a much lesser extent. While theoverall conservation of domains VI and VIII between the herpesviruskinases is low (11), all of the herpesvirus U69 homologues studiedto date have been shown to be serine/threonine protein kinases(15, 22, 37), with the exception of pseudorabies virus UL13,which has specificity for only serine residues (16). This pointsto the relatively few amino acids that are conserved within thesedomains. Of particular interest are the invariant proline (withindomain VI) which is 100% conserved in serine/threonine proteinkinases and the phenylalanine (within domain VIII) which is highlyconserved in serine/threonine protein kinases, both of which canbe found in the U69 ORF at amino acid positions 313 and 373, respectively.These amino acids may be considered essential in determining thehydroxyamino acid specificity of U69 and are therefore candidatesfor site-directed mutagenesis to investigate functional domainsof theprotein.

We compared the activities of the U69 proteins from HHV-6A and HHV-6B by using equal amounts of the proteins and observedthat autophosphorylation of HHV-6B U69 was more extensive thanthat of HHV-6A U69. HHV-6B U69 also had increased electrophoreticmobility, which has been reported to be a direct consequence ofprotein phosphorylation (20). These data suggest that HHV-6AU69 was either less efficient at autophosphorylation or had fewerphosphorylation sites than HHV-6B U69. To investigate this enzymologically,enzyme kinetic analysis of the rate of phosphorylation showedthat the K_m of HHV-6A U69 for ATP was fourfold higher than thatof HHV-6B U69. Therefore, these observations indicate that U69from HHV-6A is less efficient at autophosphorylation than U69from HHV-6B at the level of the U69-ATP interaction. It is notinconceivable that a difference in protein kinase activity existsbetween the U69 proteins because HHV-6A and HHV-6B are distinctin biology (reviewed in the introduction). DNA sequencing of theHHV-6A and HHV-6B U69 ORFs did reveal differences, but surprisingly,mutations were not found within the catalytic domains of the U69ORFs. The catalytic domains of protein kinases are important insubstrate specificity and binding (21), but other regions thatlie outside those may be important in stabilizing the overallstructure of the protein and hence contribute to the catalyticactivity. Therefore, it follows that the difference in proteinkinase activity observed between the HHV-6A and HHV-6B U69 proteinsis likely due to subtle differences in structuralstability.

The expression of U69 using a recombinant baculovirus which is otherwise relatively insensitive to GCV at noncytotoxic concentrationsrenders viral replication sensitive to the drug. This suggeststhat the U69 gene product can confer GCV sensitivity on baculovirusindependently of other HHV-6 proteins. The simplest explanationfor the mechanism of GCV phosphorylation is that U69 phosphorylatesthe drug by a direct molecular interaction between the drug andthe protein. Our data alone cannot exclude the alternative, whichis that U69 in some way activates a cellular or baculovirus proteinwhich results in GCV phosphorylation as an end product. Nevertheless,our data do demonstrate that U69 controls GCV phosphorylationin insect cells and, by implication, may carry out a similar functionin HHV-6-infected cells. The system described here will be veryhelpful to test the influence of U69 mutations on the phosphorylationof not only GCV but also other thymidine kinase-dependentdrugs.

Since the herpesvirus kinases have been postulated as being required for efficient viral replication (4, 11, 12, 36,38, 42), further studies are required to identify the cellularor viral protein targets for U69 phosphorylation. Identificationof the catalytic residues required for its protein kinase andGCV kinase activities would be important, since independent catalyticsites may facilitate the development of novel U69 protein kinaseinhibitors which could be used in conjunction with GCV as a therapeuticapproach for HHV-6.

	ACKNOWLEDGMENTS

We are very grateful to Chris G. Ullman for his help and advice throughout this project. We thank Peter Rowe for allowingaccess to the BioRad Fluoroimager, and we also thank our colleaguesPaul D. Griffiths and Duncan A. Clark for critical reading ofthemanuscript.

This research was funded by a Medical Research Council Realising Our Potential Award(UK).

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Virology, Royal Free and University College Medical School, UniversityCollege London, Royal Free Campus, Rowland Hill St., Hampstead,London NW3 2PF, United Kingdom. Phone: 44 171 794 0500, ext. 3109.Fax: 44 171 830 2854. E-mail: vincent{at}rfhsm.ac.uk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ablashi, D. V., S. Z. Salahuddin, S. F. Josephs, F. Imam, P. Lusso, R. C. Gallo, C. Hung, J. Lemp, and P. D. Markham. 1987. HBLV (or HHV-6) in human cell lines. Nature 329:207[Medline].

2. Agut, H., J. M. Huraux, H. Collandre, and L. Montagnier. 1989. Susceptibility of human herpesvirus 6 to acyclovir and ganciclovir. Lancet ii:626.

3. Asano, Y., T. Yoshikawa, S. Suga, T. Yazaki, K. Kondo, and K. Yamanishi. 1990. Fatal fulminant hepatitis in an infant with human herpesvirus-6 infection. Lancet 335:862-863[Medline].

4. Asano, Y., T. Yoshikawa, Y. Kajita, R. Ogura, S. Suga, T. Yazaki, T. Nakashima, A. Yamada, and T. Kurata. 1992. Fatal encephalitis/encephalopathy in primary human herpesvirus-6 infection. Arch. Dis. Child. 67:1484-1485[Abstract].

5. Baboonian, C., P. J. Venables, R. N. Maini, H. O. Kangro, and H. K. Osman. 1990. Antibodies to human herpesvirus-6 in Sjogren's syndrome. Arthritis Rheum. 33:1749-1750[Medline].

6. Bowen, E. F., P. Wilson, A. Cope, C. Sabin, P. Griffiths, C. Davey, M. A. Johnson, and V. Emery. 1996. Cytomegalovirus retinitis in AIDS patients: influence of cytomegaloviral load on response to ganciclovir, time to recurrence and survival. AIDS 10:1515-1520[Medline].

7. Buchwald, D., P. R. Cheney, D. L. Peterson, B. Henry, S. B. Wormsley, A. Geiger, D. V. Ablashi, S. Z. Salahuddin, C. Saxinger, and R. Biddle. 1992. A chronic illness characterized by fatigue, neurologic and immunologic disorders, and active human herpesvirus type 6 infection. Ann. Intern. Med. 116:103-113.

8. Burns, W. H., and G. R. Sandford. 1990. Susceptibility of human herpesvirus 6 to antivirals in vitro. J. Infect. Dis. 162:634-637[Medline].

9. Carrigan, D. R., W. R. Drobyski, S. K. Russler, M. A. Tapper, K. K. Knox, and R. C. Ash. 1991. Interstitial pneumonitis associated with human herpesvirus-6 infection after marrow transplantation. Lancet 338:147-149[Medline].

10. Carrigan, D. R., and K. K. Knox. 1994. Human herpesvirus 6 (HHV-6) isolation from bone marrow: HHV-6-associated bone marrow suppression in bone marrow transplant patients. Blood 84:3307-3310[Abstract/Free Full Text].

11. Chee, M. S., G. L. Lawrence, and B. G. Barrell. 1989. Alpha-, beta- and gammaherpesviruses encode a putative phosphotransferase. J. Gen. Virol. 70:1151-1160[Abstract/Free Full Text].

12. Chou, S., S. Guentzel, K. R. Michels, R. C. Miner, and W. L. Drew. 1995. Frequency of UL97 phosphotransferase mutations related to ganciclovir resistance in clinical cytomegalovirus isolates. J. Infect. Dis. 172:239-242[Medline].

13. Coulter, L. J., H. W. Moss, J. Lang, and D. J. McGeoch. 1993. A mutant of herpes simplex virus type 1 in which the UL13 protein kinase gene is disrupted. J. Gen. Virol. 74:387-395[Abstract/Free Full Text].

14. Cunningham, C., A. J. Davison, A. Dolan, M. C. Frame, D. J. McGeoch, D. M. Meredith, H. W. Moss, and A. C. Orr. 1992. The UL13 virion protein of herpes simplex virus type 1 is phosphorylated by a novel virus-induced protein kinase. J. Gen. Virol. 73:303-311[Abstract/Free Full Text].

15. Daikoku, T., S. Shibata, F. Goshima, S. Oshima, T. Tsurumi, H. Yamada, Y. Yamashita, and Y. Nishiyama. 1997. Purification and characterization of the protein kinase encoded by the UL13 gene of herpes simplex virus type 2. Virology 235:82-93[Medline].

16. de Wind, N., J. Domen, and A. Berns. 1992. Herpesviruses encode an unusual protein-serine/threonine kinase which is nonessential for growth in cultured cells. J. Virol. 66:5200-5209[Abstract/Free Full Text].

17. Di Luca, D., P. Mirandola, T. Ravaioli, B. Bigoni, and E. Cassai. 1996. Distribution of HHV-6 variants in human tissues. Infect. Agents Dis. 5:203-214[Medline].

18. Drobyski, W. R., K. K. Knox, D. Majewski, and D. R. Carrigan. 1994. Brief report: fatal encephalitis due to variant B human herpesvirus-6 infection in a bone marrow-transplant recipient. N. Engl. J. Med. 330:1356-1360[Free Full Text].

19. 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[Medline].

20. Grasser, F. A., and S. Konig. 1992. Phosphorylation of SV40 large T antigen at threonine residues results in conversion to a lower apparent molecular weight form. Arch. Virol. 126:313-320[Medline].

21. Hanks, S. K., A. M. Quinn, and T. Hunter. 1988. The protein kinase family: conserved features and deduced phylogeny of the catalytic domains. Science 241:42-52[Abstract/Free Full Text].

22. He, Z., Y. S. He, Y. Kim, L. Chu, C. Ohmstede, K. K. Biron, and D. M. Coen. 1997. The human cytomegalovirus UL97 protein is a protein kinase that autophosphorylates on serines and threonines. J. Virol. 71:405-411[Abstract].

23. Heineman, T. C., and J. I. Cohen. 1995. The varicella-zoster virus (VZV) open reading frame 47 (ORF47) protein kinase is dispensable for viral replication and is not required for phosphorylation of ORF63 protein, the VZV homolog of herpes simplex virus ICP22. J. Virol. 69:7367-7370[Abstract].

24. Herbein, G., J. Strasswimmer, M. Altieri, M. L. Woehl-Jaegle, P. Wolf, and G. Obert. 1996. Longitudinal study of human herpesvirus 6 infection in organ transplant recipients. Clin. Infect. Dis. 22:171-173[Medline].

25. Hidaka, Y., K. Kusuhara, A. Takabayashi, K. Okada, C. Miyazaki, T. Aoki, and K. Ueda. 1997. Symptomatic primary infection with human herpesvirus 6 variant A. Clin. Infect. Dis. 24:1022-1023[Medline].

26. Kawaguchi, Y., C. V. Sant, and B. Roizman. 1998. Eukaryotic elongation factor 18 is hyperphosphorylated by the protein kinase encoded by the UL13 gene of herpes simplex virus 1. J. Virol. 72:1731-1736[Abstract/Free Full Text].

27. King, L. A., and R. D. Possee. 1991. The baculovirus expression system: a laboratory guide. Chapman & Hall, New York, N.Y.

28. Knox, K. K., and D. R. Carrigan. 1994. Disseminated active HHV-6 infections in patients with AIDS. Lancet 343:577-578[Medline].

29. Knox, K. K., and D. R. Carrigan. 1996. Chronic myelosuppression associated with persistent bone marrow infection due to human herpesvirus 6 in a bone marrow transplant recipient. Clin. Infect. Dis. 22:174-175[Medline].

30. Lawrence, G. L., M. Chee, M. A. Craxton, U. A. Gompels, R. W. Honess, and B. G. Barrell. 1990. Human herpesvirus 6 is closely related to human cytomegalovirus. J. Virol. 64:287-299[Abstract/Free Full Text].

31. Levine, P. H., P. Ebbesen, D. V. Ablashi, W. C. Saxinger, A. Nordentoft, and RR Connelly. 1992. Antibodies to human herpes virus-6 and clinical course in patients with Hodgkin's disease. Int. J. Cancer 51:53-57[Medline].

32. Littler, E., A. D. Stuart, and M. S. Chee. 1992. Human cytomegalovirus UL97 open reading frame encodes a protein that phosphorylates the antiviral nucleoside analogue ganciclovir. Nature 358:160-162[Medline].

33. Lurain, N. S., L. E. Spafford, and K. D. Thompson. 1994. Mutation in the UL97 open reading frame of human cytomegalovirus strains resistant to ganciclovir. J. Virol. 68:4427-4431[Abstract/Free Full Text].

34. Lusso, P., and R. C. Gallo. 1995. Human herpesvirus 6 in AIDS. Immunol. Today 16:67-71[Medline].

35. Metzger, C., D. Michel, K. Schneider, A. Luske, H. J. Schlicht, and T. Mertens. 1994. Human cytomegalovirus UL97 kinase confers ganciclovir susceptibility to recombinant vaccinia virus. J. Virol. 68:8423-8427[Abstract/Free Full Text].

36. Michel, D., I. Pavic, A. Zimmermann, E. Haupt, K. Wunderlich, M. Heuschmid, and T. Mertens. 1996. The UL97 gene product of human cytomegalovirus is an early-late protein with a nuclear localization but is not a nucleoside kinase. J. Virol. 70:6340-6346[Abstract].

37. Ng, T. I., and C. Grose. 1992. Serine protein kinase associated with varicella-zoster virus ORF 47. Virology 191:9-18[Medline].

38. Ng, T. I., L. Keenan, P. R. Kinchington, and C. Grose. 1994. Phosphorylation of varicella-zoster virus open reading frame (ORF) 62 regulatory product by viral ORF 47-associated protein kinase. J. Virol. 68:1350-1359[Abstract/Free Full Text].

39. Overton, H. A., D. J. McMillan, L. S. Klavinskis, L. Hope, A. J. Ritchie, and P. Wong-Kai-In. 1992. Herpes simplex virus type 1 gene UL13 encodes a phosphoprotein that is a component of the virion. Virology 190:184-192[Medline].

40. Parker, C. A., and J. M. Weber. 1993. An enzyme-linked immunosorbent assay for the detection of IgG and IgM antibodies to human herpesvirus type 6. J. Virol. Methods 41:265-275[Medline].

41. 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, and T. R. Dambaugh. 1992. Primary human herpesvirus 6 infection in young children. N. Engl. J. Med. 326:1445-1450[Abstract].

42. Purves, F. C., W. O. Ogle, and B. Roizman. 1993. Processing of the herpes simplex virus regulatory protein alpha 22 mediated by the UL13 protein kinase determines the accumulation of a subset of alpha and gamma mRNAs and proteins in infected cells. Proc. Natl. Acad. Sci. USA 90:6701-6705[Abstract/Free Full Text].

43. Rosenfeld, C. S., W. B. Rybka, D. Weinbaum, D. R. Carrigan, K. K. Knox, D. F. Andrews, and R. K. Shadduck. 1995. Late graft failure due to dual bone marrow infection with variants A and B of human herpesvirus-6. Exp. Hematol. 23:626-629[Medline].

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

45. Saxinger, C., H. Polesky, N. Eby, S. Grufferman, R. Murphy, G. Tegtmeir, V. Parekh, S. Memon, and C. Hung. 1988. Antibody reactivity with HBLV (HHV-6) in U.S. populations. J. Virol. Methods 21:199-208[Medline].

46. Singh, N., and D. R. Carrigan. 1996. Human herpesvirus-6 in transplantation: an emerging pathogen. Ann. Intern. Med. 124:1065-1071[Abstract/Free Full Text].

47. Smith, I. L., J. M. Cherrington, R. E. Jiles, M. D. Fuller, W. R. Freeman, and S. A. Spector. 1997. High-level resistance of cytomegalovirus to ganciclovir is associated with alterations in both the UL97 and DNA polymerase genes. J. Infect. Dis. 176:69-77[Medline].

48. Soldan, S. S., R. Berti, N. Salem, P. Secchiero, L. Flamand, P. A. Calabresi, M. B. Brennan, H. W. Maloni, H. F. McFarland, H. C. Lin, M. Patnaik, and S. Jacobson. 1997. Association of human herpes virus 6 (HHV-6) with multiple sclerosis: increased IgM response to HHV-6 early antigen and detection of serum HHV-6 DNA. Nat. Med. 3:1394-1397[Medline].

49. Sullivan, V., C. L. Talarico, S. C. Stanat, M. Davis, D. M. Coen, and K. K. Biron. 1992. A protein kinase homologue controls phosphorylation of ganciclovir in human cytomegalovirus-infected cells. Nature 358:162-164[Medline].

50. Takahashi, K., M. Suzuki, Y. Iwata, S. Shigeto, K. Yamanishi, and E. De Clercq. 1997. Selective activity of various nucleoside and nucleotide analogues against human herpesvirus 6 and 7. Antiviral Chem. Chemother. 8:24-31.

51. Yamanishi, K., T. Okuno, K. Shiraki, M. Takahashi, T. Kondo, Y. Asano, and T. Kurata. 1988. Identification of human herpesvirus-6 as a causal agent for exanthem subitum. Lancet i:1065-1067.

52. Yoshikawa, T., T. Nakashima, S. Suga, Y. Asano, T. Yazaki, H. Kimura, T. Morishima, K. Kondo, and K. Yamanishi. 1992. Human herpesvirus-6 DNA in cerebrospinal fluid of a child with exanthem subitum and meningoencephalitis. Pediatrics 89:888-890[Abstract/Free Full Text].

53. Yoshikawa, T., S. Suga, Y. Asano, T. Nakashima, T. Yazaki, Y. Ono, T. Fujita, K. Tsuzuki, S. Sugiyama, and S. Oshima. 1992. A prospective study of human herpesvirus-6 infection in renal transplantation. Transplantation 54:879-883[Medline].

This article has been cited by other articles:

Isegawa, Y., Miyamoto, Y., Yasuda, Y., Semi, K., Tsujimura, K., Fukunaga, R., Ohshima, A., Horiguchi, Y., Yoneda, Y., Sugimoto, N. (2008). Characterization of the Human Herpesvirus 6 U69 Gene Product and Identification of Its Nuclear Localization Signal. J. Virol. 82: 710-718 [Abstract] [Full Text]
Orihara, Y., Hamamoto, H., Kasuga, H., Shimada, T., Kawaguchi, Y., Sekimizu, K. (2008). A silkworm baculovirus model for assessing the therapeutic effects of antiviral compounds: characterization and application to the isolation of antivirals from traditional medicines. J. Gen. Virol. 89: 188-194 [Abstract] [Full Text]
De Bolle, L., Naesens, L., De Clercq, E. (2005). Update on Human Herpesvirus 6 Biology, Clinical Features, and Therapy. Clin. Microbiol. Rev. 18: 217-245 [Abstract] [Full Text]
Gershburg, E., Marschall, M., Hong, K., Pagano, J. S. (2004). Expression and Localization of the Epstein-Barr Virus-Encoded Protein Kinase. J. Virol. 78: 12140-12146 [Abstract] [Full Text]
Dockrell, D.H. (2003). Human herpesvirus 6: molecular biology and clinical features. J Med Microbiol 52: 5-18 [Abstract] [Full Text]
De Bolle, L., Michel, D., Mertens, T., Manichanh, C., Agut, H., De Clercq, E., Naesens, L. (2002). Role of the Human Herpesvirus 6 U69-Encoded Kinase in the Phosphorylation of Ganciclovir. Mol. Pharmacol. 62: 714-721 [Abstract] [Full Text]
Baek, M.-C., Krosky, P. M., He, Z., Coen, D. M. (2002). Specific Phosphorylation of Exogenous Protein and Peptide Substrates by the Human Cytomegalovirus UL97 Protein Kinase. IMPORTANCE OF THE P+5 POSITION. J. Biol. Chem. 277: 29593-29599 [Abstract] [Full Text]
Manichanh, C., Olivier-Aubron, C., Lagarde, J.-P., Aubin, J.-T., Bossi, P., Gautheret-Dejean, A., Huraux, J.-M., Agut, H. (2001). Selection of the same mutation in the U69 protein kinase gene of human herpesvirus-6 after prolonged exposure to ganciclovir in vitro and in vivo. J. Gen. Virol. 82: 2767-2776 [Abstract] [Full Text]
Moore, S. M., Cannon, J. S., Tanhehco, Y. C., Hamzeh, F. M., Ambinder, R. F. (2001). Induction of Epstein-Barr Virus Kinases To Sensitize Tumor Cells to Nucleoside Analogues. Antimicrob. Agents Chemother. 45: 2082-2091 [Abstract] [Full Text]
Marschall, M., Stein-Gerlach, M., Freitag, M., Kupfer, R., van den Bogaard, M., Stamminger, T. (2001). Inhibitors of human cytomegalovirus replication drastically reduce the activity of the viral protein kinase pUL97. J. Gen. Virol. 82: 1439-1450 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Ansari, A.
	Articles by Emery, V. C.
	Search for Related Content

PubMed

	PubMed Citation

1.	Ablashi, D. V., S. Z. Salahuddin, S. F. Josephs, F. Imam, P. Lusso, R. C. Gallo, C. Hung, J. Lemp, and P. D. Markham. 1987. HBLV (or HHV-6) in human cell lines. Nature 329:207[Medline].
2.	Agut, H., J. M. Huraux, H. Collandre, and L. Montagnier. 1989. Susceptibility of human herpesvirus 6 to acyclovir and ganciclovir. Lancet ii:626.
3.	Asano, Y., T. Yoshikawa, S. Suga, T. Yazaki, K. Kondo, and K. Yamanishi. 1990. Fatal fulminant hepatitis in an infant with human herpesvirus-6 infection. Lancet 335:862-863[Medline].
4.	Asano, Y., T. Yoshikawa, Y. Kajita, R. Ogura, S. Suga, T. Yazaki, T. Nakashima, A. Yamada, and T. Kurata. 1992. Fatal encephalitis/encephalopathy in primary human herpesvirus-6 infection. Arch. Dis. Child. 67:1484-1485[Abstract].
5.	Baboonian, C., P. J. Venables, R. N. Maini, H. O. Kangro, and H. K. Osman. 1990. Antibodies to human herpesvirus-6 in Sjogren's syndrome. Arthritis Rheum. 33:1749-1750[Medline].
6.	Bowen, E. F., P. Wilson, A. Cope, C. Sabin, P. Griffiths, C. Davey, M. A. Johnson, and V. Emery. 1996. Cytomegalovirus retinitis in AIDS patients: influence of cytomegaloviral load on response to ganciclovir, time to recurrence and survival. AIDS 10:1515-1520[Medline].
7.	Buchwald, D., P. R. Cheney, D. L. Peterson, B. Henry, S. B. Wormsley, A. Geiger, D. V. Ablashi, S. Z. Salahuddin, C. Saxinger, and R. Biddle. 1992. A chronic illness characterized by fatigue, neurologic and immunologic disorders, and active human herpesvirus type 6 infection. Ann. Intern. Med. 116:103-113.
8.	Burns, W. H., and G. R. Sandford. 1990. Susceptibility of human herpesvirus 6 to antivirals in vitro. J. Infect. Dis. 162:634-637[Medline].
9.	Carrigan, D. R., W. R. Drobyski, S. K. Russler, M. A. Tapper, K. K. Knox, and R. C. Ash. 1991. Interstitial pneumonitis associated with human herpesvirus-6 infection after marrow transplantation. Lancet 338:147-149[Medline].
10.	Carrigan, D. R., and K. K. Knox. 1994. Human herpesvirus 6 (HHV-6) isolation from bone marrow: HHV-6-associated bone marrow suppression in bone marrow transplant patients. Blood 84:3307-3310[Abstract/Free Full Text].
11.	Chee, M. S., G. L. Lawrence, and B. G. Barrell. 1989. Alpha-, beta- and gammaherpesviruses encode a putative phosphotransferase. J. Gen. Virol. 70:1151-1160[Abstract/Free Full Text].
12.	Chou, S., S. Guentzel, K. R. Michels, R. C. Miner, and W. L. Drew. 1995. Frequency of UL97 phosphotransferase mutations related to ganciclovir resistance in clinical cytomegalovirus isolates. J. Infect. Dis. 172:239-242[Medline].
13.	Coulter, L. J., H. W. Moss, J. Lang, and D. J. McGeoch. 1993. A mutant of herpes simplex virus type 1 in which the UL13 protein kinase gene is disrupted. J. Gen. Virol. 74:387-395[Abstract/Free Full Text].
14.	Cunningham, C., A. J. Davison, A. Dolan, M. C. Frame, D. J. McGeoch, D. M. Meredith, H. W. Moss, and A. C. Orr. 1992. The UL13 virion protein of herpes simplex virus type 1 is phosphorylated by a novel virus-induced protein kinase. J. Gen. Virol. 73:303-311[Abstract/Free Full Text].
15.	Daikoku, T., S. Shibata, F. Goshima, S. Oshima, T. Tsurumi, H. Yamada, Y. Yamashita, and Y. Nishiyama. 1997. Purification and characterization of the protein kinase encoded by the UL13 gene of herpes simplex virus type 2. Virology 235:82-93[Medline].
16.	de Wind, N., J. Domen, and A. Berns. 1992. Herpesviruses encode an unusual protein-serine/threonine kinase which is nonessential for growth in cultured cells. J. Virol. 66:5200-5209[Abstract/Free Full Text].
17.	Di Luca, D., P. Mirandola, T. Ravaioli, B. Bigoni, and E. Cassai. 1996. Distribution of HHV-6 variants in human tissues. Infect. Agents Dis. 5:203-214[Medline].
18.	Drobyski, W. R., K. K. Knox, D. Majewski, and D. R. Carrigan. 1994. Brief report: fatal encephalitis due to variant B human herpesvirus-6 infection in a bone marrow-transplant recipient. N. Engl. J. Med. 330:1356-1360[Free Full Text].
19.	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[Medline].
20.	Grasser, F. A., and S. Konig. 1992. Phosphorylation of SV40 large T antigen at threonine residues results in conversion to a lower apparent molecular weight form. Arch. Virol. 126:313-320[Medline].
21.	Hanks, S. K., A. M. Quinn, and T. Hunter. 1988. The protein kinase family: conserved features and deduced phylogeny of the catalytic domains. Science 241:42-52[Abstract/Free Full Text].
22.	He, Z., Y. S. He, Y. Kim, L. Chu, C. Ohmstede, K. K. Biron, and D. M. Coen. 1997. The human cytomegalovirus UL97 protein is a protein kinase that autophosphorylates on serines and threonines. J. Virol. 71:405-411[Abstract].
23.	Heineman, T. C., and J. I. Cohen. 1995. The varicella-zoster virus (VZV) open reading frame 47 (ORF47) protein kinase is dispensable for viral replication and is not required for phosphorylation of ORF63 protein, the VZV homolog of herpes simplex virus ICP22. J. Virol. 69:7367-7370[Abstract].
24.	Herbein, G., J. Strasswimmer, M. Altieri, M. L. Woehl-Jaegle, P. Wolf, and G. Obert. 1996. Longitudinal study of human herpesvirus 6 infection in organ transplant recipients. Clin. Infect. Dis. 22:171-173[Medline].
25.	Hidaka, Y., K. Kusuhara, A. Takabayashi, K. Okada, C. Miyazaki, T. Aoki, and K. Ueda. 1997. Symptomatic primary infection with human herpesvirus 6 variant A. Clin. Infect. Dis. 24:1022-1023[Medline].
26.	Kawaguchi, Y., C. V. Sant, and B. Roizman. 1998. Eukaryotic elongation factor 18 is hyperphosphorylated by the protein kinase encoded by the UL13 gene of herpes simplex virus 1. J. Virol. 72:1731-1736[Abstract/Free Full Text].
27.	King, L. A., and R. D. Possee. 1991. The baculovirus expression system: a laboratory guide. Chapman & Hall, New York, N.Y.
28.	Knox, K. K., and D. R. Carrigan. 1994. Disseminated active HHV-6 infections in patients with AIDS. Lancet 343:577-578[Medline].
29.	Knox, K. K., and D. R. Carrigan. 1996. Chronic myelosuppression associated with persistent bone marrow infection due to human herpesvirus 6 in a bone marrow transplant recipient. Clin. Infect. Dis. 22:174-175[Medline].
30.	Lawrence, G. L., M. Chee, M. A. Craxton, U. A. Gompels, R. W. Honess, and B. G. Barrell. 1990. Human herpesvirus 6 is closely related to human cytomegalovirus. J. Virol. 64:287-299[Abstract/Free Full Text].
31.	Levine, P. H., P. Ebbesen, D. V. Ablashi, W. C. Saxinger, A. Nordentoft, and RR Connelly. 1992. Antibodies to human herpes virus-6 and clinical course in patients with Hodgkin's disease. Int. J. Cancer 51:53-57[Medline].
32.	Littler, E., A. D. Stuart, and M. S. Chee. 1992. Human cytomegalovirus UL97 open reading frame encodes a protein that phosphorylates the antiviral nucleoside analogue ganciclovir. Nature 358:160-162[Medline].
33.	Lurain, N. S., L. E. Spafford, and K. D. Thompson. 1994. Mutation in the UL97 open reading frame of human cytomegalovirus strains resistant to ganciclovir. J. Virol. 68:4427-4431[Abstract/Free Full Text].
34.	Lusso, P., and R. C. Gallo. 1995. Human herpesvirus 6 in AIDS. Immunol. Today 16:67-71[Medline].
35.	Metzger, C., D. Michel, K. Schneider, A. Luske, H. J. Schlicht, and T. Mertens. 1994. Human cytomegalovirus UL97 kinase confers ganciclovir susceptibility to recombinant vaccinia virus. J. Virol. 68:8423-8427[Abstract/Free Full Text].
36.	Michel, D., I. Pavic, A. Zimmermann, E. Haupt, K. Wunderlich, M. Heuschmid, and T. Mertens. 1996. The UL97 gene product of human cytomegalovirus is an early-late protein with a nuclear localization but is not a nucleoside kinase. J. Virol. 70:6340-6346[Abstract].
37.	Ng, T. I., and C. Grose. 1992. Serine protein kinase associated with varicella-zoster virus ORF 47. Virology 191:9-18[Medline].
38.	Ng, T. I., L. Keenan, P. R. Kinchington, and C. Grose. 1994. Phosphorylation of varicella-zoster virus open reading frame (ORF) 62 regulatory product by viral ORF 47-associated protein kinase. J. Virol. 68:1350-1359[Abstract/Free Full Text].
39.	Overton, H. A., D. J. McMillan, L. S. Klavinskis, L. Hope, A. J. Ritchie, and P. Wong-Kai-In. 1992. Herpes simplex virus type 1 gene UL13 encodes a phosphoprotein that is a component of the virion. Virology 190:184-192[Medline].
40.	Parker, C. A., and J. M. Weber. 1993. An enzyme-linked immunosorbent assay for the detection of IgG and IgM antibodies to human herpesvirus type 6. J. Virol. Methods 41:265-275[Medline].
41.	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, and T. R. Dambaugh. 1992. Primary human herpesvirus 6 infection in young children. N. Engl. J. Med. 326:1445-1450[Abstract].
42.	Purves, F. C., W. O. Ogle, and B. Roizman. 1993. Processing of the herpes simplex virus regulatory protein alpha 22 mediated by the UL13 protein kinase determines the accumulation of a subset of alpha and gamma mRNAs and proteins in infected cells. Proc. Natl. Acad. Sci. USA 90:6701-6705[Abstract/Free Full Text].
43.	Rosenfeld, C. S., W. B. Rybka, D. Weinbaum, D. R. Carrigan, K. K. Knox, D. F. Andrews, and R. K. Shadduck. 1995. Late graft failure due to dual bone marrow infection with variants A and B of human herpesvirus-6. Exp. Hematol. 23:626-629[Medline].
44.	Salahuddin, S. Z., D. V. Ablashi, P. D. Markham, S. F. Josephs, S. Sturzenegger, M. Kaplan, G. Halligan, P. Biberfeld, F. Wong-Staal, and B. Kramarsky. 1986. Isolation of a new virus, HBLV, in patients with lymphoproliferative disorders. Science 234:596-601[Abstract/Free Full Text].
45.	Saxinger, C., H. Polesky, N. Eby, S. Grufferman, R. Murphy, G. Tegtmeir, V. Parekh, S. Memon, and C. Hung. 1988. Antibody reactivity with HBLV (HHV-6) in U.S. populations. J. Virol. Methods 21:199-208[Medline].
46.	Singh, N., and D. R. Carrigan. 1996. Human herpesvirus-6 in transplantation: an emerging pathogen. Ann. Intern. Med. 124:1065-1071[Abstract/Free Full Text].
47.	Smith, I. L., J. M. Cherrington, R. E. Jiles, M. D. Fuller, W. R. Freeman, and S. A. Spector. 1997. High-level resistance of cytomegalovirus to ganciclovir is associated with alterations in both the UL97 and DNA polymerase genes. J. Infect. Dis. 176:69-77[Medline].
48.	Soldan, S. S., R. Berti, N. Salem, P. Secchiero, L. Flamand, P. A. Calabresi, M. B. Brennan, H. W. Maloni, H. F. McFarland, H. C. Lin, M. Patnaik, and S. Jacobson. 1997. Association of human herpes virus 6 (HHV-6) with multiple sclerosis: increased IgM response to HHV-6 early antigen and detection of serum HHV-6 DNA. Nat. Med. 3:1394-1397[Medline].
49.	Sullivan, V., C. L. Talarico, S. C. Stanat, M. Davis, D. M. Coen, and K. K. Biron. 1992. A protein kinase homologue controls phosphorylation of ganciclovir in human cytomegalovirus-infected cells. Nature 358:162-164[Medline].
50.	Takahashi, K., M. Suzuki, Y. Iwata, S. Shigeto, K. Yamanishi, and E. De Clercq. 1997. Selective activity of various nucleoside and nucleotide analogues against human herpesvirus 6 and 7. Antiviral Chem. Chemother. 8:24-31.
51.	Yamanishi, K., T. Okuno, K. Shiraki, M. Takahashi, T. Kondo, Y. Asano, and T. Kurata. 1988. Identification of human herpesvirus-6 as a causal agent for exanthem subitum. Lancet i:1065-1067.
52.	Yoshikawa, T., T. Nakashima, S. Suga, Y. Asano, T. Yazaki, H. Kimura, T. Morishima, K. Kondo, and K. Yamanishi. 1992. Human herpesvirus-6 DNA in cerebrospinal fluid of a child with exanthem subitum and meningoencephalitis. Pediatrics 89:888-890[Abstract/Free Full Text].
53.	Yoshikawa, T., S. Suga, Y. Asano, T. Nakashima, T. Yazaki, Y. Ono, T. Fujita, K. Tsuzuki, S. Sugiyama, and S. Oshima. 1992. A prospective study of human herpesvirus-6 infection in renal transplantation. Transplantation 54:879-883[Medline].