Identification and Analysis of the K5 Gene of Kaposi's Sarcoma-Associated Herpesvirus

doi:10.1128/JVI.74.6.2867-2875.2000

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Journal of Virology, March 2000, p. 2867-2875, Vol. 74, No. 6
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Identification and Analysis of the K5 Gene of Kaposi's Sarcoma-Associated Herpesvirus

Muzammel Haque,¹ Jiguo Chen,¹ Keiji Ueda,¹ Yasuko Mori,¹ Kazusi Nakano,¹ Yuko Hirata,¹ Shiro Kanamori,² Yasuo Uchiyama,² Reiko Inagi,¹ Toshiomi Okuno,³ and Koichi Yamanishi¹^,^*

Department of Microbiology¹ and Department of Cell Biology and Neurosciences,² Osaka University Medical School C1, 2-2 Yamadaoka, Suita 565-0871, and Department of Microbiology, Hyogo Medical College, Nishinomiya 663-8131, Hyogo,³ Japan

Received 13 September 1999/Accepted 2 December 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Kaposi's sarcoma-associated herpesvirus (KSHV), or human herpesvirus 8 (HHV-8), belongs to the gammaherpesvirus subfamilyand encodes ~80 open reading frames (ORFs). Among them are a fewcandidates for immediate-early genes (e.g., K5). We developeda monoclonal antibody (MAb), 328C7, against the K5 antigen. ThisMAb reacted with the K5 gene product by immunoscreening of a cDNAlibrary from BCBL-1 cells, and this result was confirmed by transfectionof the K5 ORF into Cos-7 cells. After induction of lytic infectionby treatment with 12-O-tetradecanoylphorbol-13-acetate, MAb 328C7reacted with an antigen in the cytoplasm of BCBL-1 and BC-3 cellsas early as after 4 h of induction. Immunoelectron microscopyshowed that the K5 antigen was situated mainly in the endoplasmicreticulum but was not present on the virion or in the nucleus.Northern blotting with a K5-specific probe revealed a single transcriptof 1.2 kb, while Western blotting showed the antigen to be a 36-kDapolypeptide. The 5' and 3' ends were then determined by rapidamplification of cDNA, followed by sequencing of RACE products,and a splice was revealed upstream of the K5 ORF. K5 expressionwas unaffected by the respective DNA and protein synthesis inhibitorsphosphonoformic acid and cycloheximide plus actinomycin D, confirmingits immediate-early nature. Transient-transfection assays showedthat the K5 promoter was transactivated by ORF 50 (KSHV Rta),a homolog of Epstein-Barr virus Rta, but the K5 gene product exhibitedno transregulation of its own promoter or those of DNA polymeraseand the human immunodeficiency virus type 1 long terminal repeat.This is the first such analysis of an immediate-early gene product;determination of its specific biological function requires furtherinvestigation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Kaposi's sarcoma-associated herpesvirus (KSHV), or human herpesvirus 8 (HHV-8), was recently discovered in tissues isolatedfrom varied forms of Kaposi's sarcoma (7, 18, 38), Castleman'sdisease (39), and body cavity-based lymphoma (BCBL; primaryeffusion lymphoma) (5). The etiology and pathogenic mechanismsof HHV-8 are as yet unknown, but its origin and kindred stronglysuggest that HHV-8 promotes a particular type of cell proliferation(28). All of the cell lines derived from BCBL harbor the HHV-8genome in a latent state; the virus is transformed to a lyticstate by chemical agents such as 12-O-tetradecanoylphorbol-13-acetate(TPA) and n-butyrate (1, 5, 24, 25, 34, 37). Thefirst such cell line reported, BC-1, was also infected with Epstein-Barrvirus (EBV) (6, 13), but later BCBL lines were EBV negative(1, 34). Although HHV-8 is difficult to transmit, it canbe maintained in some cell lines and virus production can be inducedby treatment with TPA or n-butyrate (12, 27).

HHV-8 is a new member of the gammaherpesvirus subfamily and has genetic similarity to herpesvirus saimiri (HVS) and EBV (27,35). Its genome, which has been completely sequenced, consistsof a double-stranded long unique DNA sequence of 140.5 kbp flankedby GC-rich terminal repeat sequences (30, 35). It encodesabout 80 complete open reading frames (ORFs), some of which havesimilarity to those of HVS (35). Among them, 15 ORFs, designatedK1 to K15, are unique to HHV-8. In addition, HHV-8 encodes a numberof human gene homologs related to immune function and cell cycleregulation, including ORFs 16 (viral Bcl-2) (8, 36), 72 (viralcyclin D) (14, 21, 33), 74 (viral interleukin-8 receptor)(2, 16), K2 (viral interleukin-6) (4, 26, 30, 31),K4 and K6 (viral macrophage inflammatory proteins I and II, respectively)(3, 20, 31), K9 (viral interferon regulatory factor) (19,22, 47), and K13 (vFLIP/vFLICE [caspase-8]-inhibitory protease)(42). Earlier reports suggested that some of these factors do,indeed, initiate cell proliferation, thereby promoting tumorprogression.

Herpesvirus genes are classified as latent, immediate-early (IE), early (E), and late (L) (17, 41, 46). Expression ofthe IE and E genes is independent of viral DNA replication, andsome are involved in gene regulation and DNA replication (17,23, 40). The L genes, by contrast, are dependent on viralDNA replication and mainly encode structural proteins (17).Regulation of gene expression in cells infected with herpesvirusesis generally ordered in a cascade fashion: IE genes are transcribedfirst following cell penetration of the virus, after which theE and L genes are expressed. Recent analysis of the complete DNAsequence suggests that HHV-8 possesses several IE candidate genes,including K3, K5, K8, ORF 45, ORF 50, and ORF 57 (35). Of these,the K3 and K5 genes have homology to the IE-1 gene from bovineherpesvirus 4 (BHV-4) (35), which is also a gammaherpesvirus(9).

To analyze HHV-8 gene function more precisely, we developed monoclonal antibodies (MAbs) against viral proteins and attemptedto identify their antigens using the $lambda$ gt11 cDNA library of HHV-8-infectedBCBL-1 cells. Among our MAbs, six specifically recognized theK5 gene product and we have used one of them (MAb 328C7) as aprobe to characterize the K5 gene and its product. To our knowledge,this is the first such analysis of a candidate IE geneproduct.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell lines and cell culture. BCBL-1 (34) or BC-3 (1) cells, which harbor HHV-8, and BC-1 cells (6), which harbor both EBV and HHV-8, were grownin RPMI 1640 medium supplemented with 10 or 20% heat-inactivatedfetal calf serum (FCS), penicillin, and streptomycin at 37°C underan atmosphere of 95% air and 5% CO₂. B95-8 and Raji cells, whichharbor EBV, and uninfected Ramos cells, a human B-cell line, werecultured in RPMI 1640 medium supplemented with 10% FCS, penicillin,and streptomycin. The latter three cell lines served as controlsthroughout the study. When necessary, lytic gene expression wasinduced in HHV-8-infected and control cells by treatment withTPA (Sigma) at 20 ng/µl. Cos-7 and 293T cells were maintainedin Dulbecco modified Eagle medium supplemented with 10% FCS, penicillin,and streptomycin and were used for transient-transfection andcotransfection assays,respectively.

Establishment and characterization of MAbs. BALB/c mice were immunized with lysates from 10⁷ TPA-induced BCBL-1 cells. The first immunization was carried out with a mixtureof cell lysates in complete Freund's adjuvant. That was followedby two or three boosters, 3 to 4 weeks apart, in incomplete Freund'sadjuvant. Three to 4 days prior to cell fusion, 10⁷ TPA-induced BCBL-1 cells in 500 µl of phosphate-buffered saline(PBS) were administeredintraperitoneally.

Hybridomas were established by fusing splenocytes from the hyperimmune mice with a nonproducing myeloma cell line, Sp-2/0-Ag14.After selection in medium containing hypoxanthine-aminopterin-thymidine,cells secreting MAbs were screened by indirect immunofluorescenceassays (IFA; see below for details). TPA-induced and uninducedBCBL-1 cells were fixed in acetone and exposed to supernatantsof the hybrid cells. Clones secreting antibodies reactive withTPA-induced BCBL-1 cells were expanded and cloned twice more bylimiting dilutions. Ascites fluids with high antibody titers werethen accumulated by injecting cloned hybrid cells intraperitoneallyinto Pristane (Sigma)-treatedmice.

IFA. BCBL-1, BC-3, and BC-1 cells were kept uninduced or induced with TPA. At selected times after induction, cells were harvested,washed twice with PBS, spotted onto slide glass in 24-well plates,air dried, and fixed with acetone for 20 min at $-$ 20°C. The fixedcells were incubated with hybridoma supernatants for 30 min atroom temperature in a humid chamber. After washing with PBS containing0.05% Tween 20 for 10 min, the slides were air dried and incubatedfor another 30 min with appropriately diluted fluorescein isothiocyanate(FITC)-conjugated goat anti-mouse immunoglobulin G (IgG; DAKO,Copenhagen, Denmark). After being washed once again as describedabove, the slides were mounted with 50% glycerol in PBS and signalswere detected by fluorescencemicroscopy.

Confocal immunohistochemistry. BCBL-1 cells were induced with TPA for 24 h, washed in PBS, spotted onto slide glass, air dried, and fixed with acetone asdescribed for the IFA. They were then incubated with a primaryanti-K5 MAb for 30 min, followed by a 1:100 dilution of FITC-conjugatedgoat anti-mouse IgG and Hoechst 33342 for another 30 min at 37°C.Specific immunofluorescence was observed under a confocal laserscanning microscope (Carl Zeiss Co. Ltd.).

Immunoelectron microscopy. BCBL-1 cells were induced with TPA for 24 h, washed with PBS, and fixed in 0.1% glutaraldehyde and 4% paraformaldehyde bufferedin 0.1 M phosphate buffer (pH 7.4) for 10 min, after which theywere fixed for an additional 12 h in 4% paraformaldehyde. To determinethe exact localization of the antigen, we used the cryo-thin-sectionimmunogold method (15). The specimens were immersed in 1.89M sucrose with 20% polyvinylpyrrolidone and frozen with liquidnitrogen. Thin frozen sections were then cut with a microtome(ULTRACUTS; Reichert-Nissei, Tokyo, Japan) and mounted on Formvarcarbon-coated nickel grids. The sections were rinsed with PBSand then Tris-buffered saline containing 1% bovine serum albuminand incubated overnight with MAb 328C7 in Tris-buffered saline.The following day, the cells were incubated for 1 h with anti-mouseIgG conjugated with 5-nm colloidal gold particles, fixed againin 2% glutaraldehyde in PBS, postfixed with 1% OsO₄, and stainedwith uranyl acetate. After dehydration in ethanol, the sectionswere embedded in LR white (London Resin.) and observed using aHitachi H-7100 electronmicroscope.

Western blot analysis. Cell lysates in Laemmli's buffer were prepared from TPA-induced and uninduced BCBL-1, BC-3, and Raji cells 24 h after induction.Samples were subjected to sodium dodecyl sulfate-10% polyacrylamidegel electrophoresis (SDS-PAGE) under reducing conditions and thenelectrophoretically transferred to polyvinylidene difluoride membranes(Bio-Rad, Hercules, Calif.) using standard procedures (19).The membranes were then blocked for 1 h while shaking at roomtemperature in PBS containing 0.05% Tween 20 and 5% skim milk,after which they were incubated with the primary antibody (1:1,000dilution of ascitic fluid in PBS-0.05% Tween 20-2% skim milk)for an additional 1 h while again shaking at room temperature.The membranes were then washed three times for 10 min each in0.05% Tween 20 in PBS and finally incubated for 1 h as describedabove with an appropriate dilution of alkaline phosphatase-conjugatedgoat anti-mouse IgG (Bio-Rad). After washing, bound enzyme-labeledMAb was detected with 5-bromo-4-chloro-3-indolylphosphate (BCIP)and nitroblue tetrazolium substrate (Wako Chemicals, Osaka,Japan).

Construction of a cDNA library and immunoscreening with anti-HHV-8 MAb. Construction of a cDNA library from BCBL-1 cells was described previously (19). This library was screened with MAb 328C7using a picoBlue Immunoscreening Kit (Stratagene) in accordancewith the manufacturer's instructions. Briefly, 5 × 10⁴ PFU of recombinant phages per 150-mm-diameter agar plate weremixed with Escherichia coli Y1090 and plated. After incubationat 37°C for 6 to 7 h, expression of fusion proteins was inducedby overlaying 10 mM IPTG-treated nitrocellulose membranes. Themembranes were blocked for 1 h in buffer containing 20 mM Tris-HCl(pH 7.5)-150 mM NaCl-1% bovine serum albumin and then reactedwith the MAb. Following incubation with an appropriate dilutionof alkaline phosphatase-conjugated goat anti-mouse IgG, reactivitywas detected with BCIP and nitroblue tetrazolium as describedfor Western blotting. Immunoreactive phages were collected, diluted,replated, and isolated by subsequent screening until they wereclonally pure. Four immunoreactive phages were then selected andrescreened through three cycles of cloning. Purified recombinantphages were transferred to SM buffer, and cDNA inserts were amplifiedby PCR and cloned into TA cloning vector pCR2.1(Invitrogen).

Analysis of the DNA sequence. The cDNA subcloned into pCR2.1 was sequenced using SequiTherm EXCEL long-read DNA sequencing kit-LC (Epicentre Technologies).DNA sequence data were compiled, and homology was analyzed bysearching data banks using FASTA and BLASTsoftware.

Construction of plasmids. The viral DNA from HHV-8-harboring BCBL-1 cells was used as a template for all PCR amplifications. The HHV-8 K5 gene fragmentwas amplified by PCR using primers with NheI and XhoI restrictionsites at the 5' and 3' ends, respectively. The amplified productswere digested with NheI and XhoI and inserted into pcDNA3.1(+)/Zeo(Invitrogen) to create plasmid pcDNA3-K5. To construct plasmidpcDNA3-KSHV/Rta, a gene fragment encoding KSHV Rta was amplifiedby PCR, digested with XbaI, and inserted into the XbaI site ofpcDNA3.1. Luciferase reporter plasmids pk5-Luc and p8pol-Luc wereconstructed by PCR amplification of fragments extending 1 kbpupstream of the respective genes relative to their translationstart (ATG) codons. The amplified products were digested withSacI and NcoI and cloned into pGL3-Basic vectors (Promega) previouslydigested with the same enzymes. Construction of a heterologousreporter plasmid containing the human immunodeficiency virus type1 (HIV-1) long terminal repeat (LTR) (PLTR-Luc) was describedpreviously (30).

Transient expression in Cos-7 cells. Prior to transfection, 4 × 10⁵ Cos-7 cells were seeded onto 60-mm-diameter dishes and incubated for 16 h at 37°C in a 5% CO₂incubator. They were then transfected with expression plasmidpcDNA3-K5 using SuperFect Transfection Reagent (Qiagen) in accordancewith the manufacturer's instructions. Twenty-four hours aftertransfection, cells were washed in PBS, collected by trypsinization,again washed in PBS, and fixed for 20 min in cold acetone at $-$ 20°C.Expression of K5 was then detected as described for confocal immunohistochemistryof BCBL-1cells.

RT-PCR and nested PCR. Reverse transcription (RT)-PCR was carried out on poly(A)⁺ RNA extracted from TPA-induced and uninduced BCBL-1 cells usingSuperscript II reverse transcriptase (GIBCO Bethesda ResearchLaboratories [BRL]), essentially as indicated in the manufacturer'sinstructions. Briefly, RT of 0.5 µg of poly(A)⁺ RNA was performed at 42°C for 50 min in a 20-µl reaction mixturecontaining 1 µl of Superscript II reverse transcriptase and 0.5µM primer AP (5'-GGCCA CGCGT CGACT AGTAC TTTTT TTTTT TTTTT TT-3')(provided in the kit). Thereafter, 2 µl of the reaction mixturewas amplified by PCR using primers K5-F (5'-TGGAC GGGCA CGAAGCGTTG AT-3') and AUAP (5'-GGCCA CGCGT CGACT AG-TAC-3') (providedin the kit). Nested PCR was carried out using 5 µl of 1:100 dilutedRT-PCR mixture and primers K5-F and K5R3 (5'-AGAAT GTTCC CGCAGGAGCA GTTAG GATGA-3'). Control reactions were carried out usinggenomic HHV-8 DNA as atemplate.

5' and 3' RACE. All primers used for cDNA synthesis and PCR were designed on the basis of cDNA sequence data from the HHV-8 cDNA library.3' and 5' rapid amplification of cDNA ends (RACE) was performedusing a cDNA ends amplification kit (GIBCO BRL) and poly(A)⁺ RNA extracted from uninduced and TPA-induced BCBL-1 cells. Thefirst-strand cDNA of 3' RACE was synthesized using SuperscriptII reverse transcriptase and an oligo(dT) primer provided withthe kit. The cDNA was amplified by PCR using an adapter-specificprimer also provided in the kit and an HHV-8-specific primer (K5F1)corresponding to the ORF K5 3' end (5'-GACTT AGGGG GACAG CGCGTACCGA CCTAT-3'). The first-strand cDNA of 5' RACE was synthesizedusing HHV-8-specific primer K5R1 (5'-GTCAC CCGGG TGTTAT TTGCCGCGTA TAAT-3') and tailed with dCTP. The cDNA was amplified byPCR using an adapter-specific primer provided in the kit and asecond HHV-8-specific primer (K5R2) corresponding to the ORF K55' end (5'-CACTT ACGCG GCATA TGCCG CCAAA TGCAA-3'). Both 3' and5' RACE cDNA PCR products were cloned into the pCR2.1 vector (Invitrogen)in accordance with the manufacturer's instructions and sequenced.The TA clones of the 3' and 5' RACE PCR products were sequencedusing a SequiTherm EXCEL sequencing kit (EPICENTRE TECHNOLOGIES)based on the dideoxynucleotide termination method, and sequenceanalyses were carried out by comparison with the published HHV-8sequence data (35).

Primer extension. Oligonucleotide primer K5R4 (5'-TACGT CCTTG GACGC CATCT-3') was 5' end labeled with IRD41 (Aloka), creating a dye primer.Ten micrograms each of poly(A)⁺ RNA extracted from TPA-induced and uninduced BCBL-1 cells wasthen mixed with 5 µl of 1 µM K5R4 dye primer, heated to 70°C for10 min, and then immediately transferred to a 50°C chamber, wherethe extension reaction was carried out for 50 min in a total volumeof 50 µl, which included 200 U of Superscript II reverse transcriptase(GIBCO BRL). After digestion with an RNase mixture for 30 minat 37°C, the samples were precipitated with ethanol and analyzedon 6% polyacrylamide sequencing gels containing 8 M urea and ona Li-Cor DNA sequencer (model 4000; Aloka). Sequence reactionsusing the same labeled primer were run in parallel experimentsusing a cDNA clone as a template to verify the size of theprimer.

Time course of K5 antigen expression. The kinetics of HHV-8 gene expression were examined in uninduced and TPA-induced BC-3 and BCBL-1 cells. To analyze K5 expression,cells were harvested and washed in PBS 2, 4, 5, 6, 8, and 12 hafter induction, spotted onto antigen plates, and permeabilizedwith acetone for IFA using MAb 328C7 as a probe. For comparison,the early gene K9 (19) was similarly analyzed using MAbB291.

Northern blotting. BCBL-1 cells (1 × 10⁷ to 2 × 10⁷) were induced for 12 h with TPA alone, TPA plus the DNA synthesis inhibitor phosphonoformicacid (PFA; 200 µg/ml), or TPA plus cycloheximide (CHX), a proteinsynthesis inhibitor, at 10 to 100 µg/ml. Total RNA was then isolatedfrom the cells using a total RNA purification kit (Qiagen) inaccordance with the manufacturer's instructions. After ethanolprecipitation, the RNA was stored at $-$ 70°C for further use. ForNorthern blot hybridization, 20 µg of total RNA was subjectedto electrophoresis on 1% agarose-formaldehyde gels, blotted ontoHybond-N nylon membranes (Amersham), and hybridized to an oligonucleotideprobe specific for the K5 gene (5'-CCCGC AGGAG CAGTT AGGAT GACCAGGAGC-3') at 42°C in a 25 mM sodium phosphate buffer containing5× SSC (1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate) and5× Denhardt's solution. After hybridization, the membranes werewashed at 42°C in solutions of decreasing ionic strength (2× SSC-0.1%SDS and 1× SSC-0.1% SDS) for 30 min each time and then exposedto Kodak XAR film with an intensifying screen. A $beta$ -actin probe(5'-AGCATTTGCGGTGGACGATGGAG-3') was used as a control. An antisenseoligonucleotide probe specific for the K9 gene (5'-TTGGCCTGGGTCCATTGTCC-3')was also used to detect the K9 transcript on the same filter.Antisense oligonucleotides were 5' labeled with T4 polynucleotidekinase and [ $gamma$ -³²P]ATP using a Mega label kit (Boehringer, Mannheim,Germany).

Metabolic labeling and immunoprecipitation. BCBL-1 cells (5 × 10⁶) were washed twice with PBS and resuspended in Dulbecco's modified Eagle medium (DMEM; GIBCO BRL) supplementedwith 5% dialyzed FCS without methionine. To differentiate HHV-8IE and E gene products, BCBL-1 cells were induced for 12 h withTPA alone or with TPA plus PFA (300 µg/ml). The cells were labeledwith [³⁵S]methionine at 220 µCi/ml during the final 1 h. As a control,uninduced BCBL-1 cells were labeled for the sameperiod.

Sequential application of metabolic inhibitors enabled us to demonstrate the true IE nature of the K5 gene product. A sampleof BCBL-1 cells (5 × 10⁷) was divided into two aliquots that were resuspended in DMEM,induced for 4 h with TPA in the presence of CHX, an inhibitorof protein synthesis, at 100 µg/ml, and cultured. One aliquotwas then washed three times with PBS to remove the CHX, resuspendedfor an additional 6 h in labeling medium containing TPA plus actinomycinD (AcD), an mRNA synthesis inhibitor, at 10 µg/ml, and cultured.CHX- and AcD-treated cells were each labeled with [³⁵S]methionine as described above, after which they were harvested,washed with PBS, lysed for 30 min on ice in RIPA buffer (0.05M Tris-HCl [pH 8.0], 0.15 M NaCl, 0.5% sodium deoxycholate, 1%Triton X-100, 0.1% SDS), and centrifuged at 13,000 × g for 15min. The resultant supernatant was then used for immunoprecipitationassays asfollows.

Two microliters of MAb 328C7 containing ascites fluid was mixed with 200 µl of protein G-Sepharose 4 FF (Pharmacia Biotech)beads and incubated at 4°C for 3 h while rotating. The beads werethen washed six times with RIPA buffer to remove unbound proteinand isotope. The radiolabeled cell lysate was mixed with proteinG-Sepharose antibody complex and rotated overnight as describedabove. After extensive washing with RIPA buffer, the immunoprecipitatewas eluted by boiling in Laemmli's buffer, separated by SDS-10%denaturing PAGE, and analyzed byfluorography.

Transregulation assay. Prior to transfection, 293T cells were plated to a density of 5 × 10⁵ cells per 60-mm-diameter tissue culture dish in DMEM supplementedwith 10% FCS and allowed to grow overnight at 37°C in a 5% CO₂incubator. Transient cotransfection was accomplished by usingSuperFect Transfection Reagent (Qiagen). A 4-µg sample of totalDNA was used for each 60-mm dish with 1 µg of reporter and 2 µgof effector plasmid, and the total quantity of transfected DNAwas kept constant by adding an appropriate amount of pcDNA3.1.Cells were harvested 24 h after transfection, and luciferase activitywas assayed. Values were normalized to the protein concentrationusing a Bio-Rad protein assay with bovine serum albumin as thestandard.

Nucleotide sequence accession number. The nucleotide sequence reported here has been deposited in the GenBank database and assigned accession no. AF117253.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

A protein specific for HHV-8-infected cells is recognized by MAb 328C7. In order to identify individual HHV-8 proteins, we raised several MAbs against whole-cell lysates of TPA-induced BCBL-1 cells.From a list of six MAbs specifically recognizing the K5 gene,in this study we used one of them, named MAb 328C7, to analyzethe K5 gene. Using IFA, MAb 328C7 was observed to react with anantigen apparently present in the cytoplasm of BCBL-1 cells (Fig.1a and b). Although only 4 to 5% of uninduced cells exhibitedspecific staining, the percentage of positive cells increasedto 80 to 90% after TPA treatment. The staining was specific forHHV-8-infected cells: Raji (Fig. 1c), B95-8, and Ramos cells (notshown) were all not stained specifically by MAb 328C7.

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FIG. 1. Fluorescence (FITC) photomicrographs showing MAb 328C7 immunoreactivity in HHV-8-infected, uninfected, and transfected cells after selected periods of induction or after transfection. BCBL-1 and Raji cells were fixed and labeled after 12 and 24 h of exposure to TPA, respectively; pcDNA3-K5-transfected Cos-7 cells were fixed and labeled 24 h posttransfection. a, untreated BCBL-1 cells; b, TPA-treated BCBL-1 cells; c, TPA-treated Raji cells; d, TPA-treated BCBL-1 cells; e, Cos-7 cells transfected with pcDNA3-K5 also stained with Hoechst 33342.

To more accurately localize K5 protein, TPA-induced BCBL-1 cells and K5-transfected Cos-7 cells were double labeled with MAb328C7 and Hoechst 33342 and examined under a confocal imagingmicroscope. Figure 1d and e shows that antigen was, indeed, distributedin the cytoplasm of induced and transfected cells, appearing asdots. The greater resolution achieved with immunoelectron microscopyusing MAb 328C7 revealed that the antigen was localized particularlyin the endoplasmic reticulum (Fig. 2A and B) but not in the nucleusand mitochondria, suggesting that the K5 protein is not a structuralprotein.

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FIG. 2. Electron micrographs demonstrating the presence of K5 antigen in BCBL-1 cells. Immunogold labeling (arrows) is detected only on membranes of endoplasmic reticulum-like structures (A and B) but not in a nucleus (N) and mitochondria (M). Immunogold labeling was performed using cryo-thin sections (gold particles, 5 nm in diameter). Original magnifications: A, ×57,000; B, ×60,000.

MAb 328C7 recognizes the K5 gene product in HHV-8-infected cells. To identify a coding gene for the protein recognized by MAb 328C7, the cDNA library constructed from TPA-induced BCBL-1 cellswas immunoscreened with the MAb. Proteins from four cDNA clonesreacted with MAb 328C7, and in each clone, the size of the insertedcDNA was approximately 0.8 to 1.0 kbp. The clone with the longestcDNA insert was sequenced and compared with the previously publishedHHV-8 sequence (35); the sequence was found to be identicalto that part of the HHV-8 sequence encoding ORF K5 (data not shown).The sequences of the 5' and 3' ends of the other three cDNA insertsoverlapped those of the K5clone.

To confirm that the antigen recognized by MAb 328C7 and the K5 protein was the same K5 ORF was amplified by PCR, insertedinto pcDNA, and transfected into Cos-7 cells. MAb 328C7 specificallyrecognized the expressed K5 protein located in the cytoplasm ofthe transfectants (Fig. 1e).

MAb 328C7 recognizes a 36-kDa protein in Western blots. To identify the viral protein recognized by the anti-K5 MAb, we performed Western blot analysis. Figure 3 shows that MAb 328C7recognized a 36-kDa polypeptide in BCBL-1 cells, and this bandwas more intensively recognized in cells treated with TPA thanin untreated ones (Fig. 3, lanes 1 and 2). It has no reactivitywith any polypeptides obtained from EBV-infected Raji cells (Fig.3, lane 3) or from uninfected cell lines (data not shown). Thus,synthesis of this antigen appears to be highly dependent on inductionof HHV-8 infection.

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FIG. 3. Western blot analysis of cell lysates obtained from TPA-treated (lane 1) and untreated (lane 2) BCBL-1 cells and untreated Raji cells (lane 3) using MAb 328C7 as a probe. Polypeptides were separated by SDS-10% PAGE under reducing conditions, transferred to a polyvinylidene difluoride membrane, and reacted with MAb 328C7. Molecular mass markers are shown on the left. The arrow indicates the HHV-8-specific polypeptide recognized by MAb 328C7.

Analysis of K5 gene transcription. When sequencing of the 5' RACE products was carried out, based on the sequence data from the cDNA library, it was found thatan mRNA with a splice occurring in the 5' noncoding region wastranscribed from the K5 locus of HHV-8 (see Fig. 6). To confirmthe 5' RACE results, RT-PCR and subsequent nested PCR were carriedout with RNA extracted from BCBL-1 cells; extracted DNA servedas a control against detection of genomic DNA using the K5F andK5R3 primers (Fig. 4A). Amplification of HHV-8 genomic DNA yieldeda 610-nucleotide fragment, as predicted by HHV-8 sequence data(Fig. 4, lane 3); however, a fragment of only about 440 nucleotideswas amplified by RT-PCR and nested PCR from RNA extracted fromTPA-treated or untreated BCBL-1 cells (Fig. 4, lanes 1 and 2,respectively).

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FIG. 4. RT-PCR and nested PCR of K5. Using DNase I-digested poly(A) RNA extracted from untreated and TPA-treated BCBL-1 cells, a spliced fragment encoding K5 was amplified by RT-PCR and subsequent nested PCR. (A) Schematic representation of the primers used in the assays. (B) Nested PCR results obtained with primers K5F and K5R3. Lanes: M, molecular weight markers ( $phi$ X174 HaeIII digest); 1, untreated cells; 2, TPA-treated cells; 3, control PCR with HHV-8 genomic DNA.

To map precisely the 5' end of the K5 transcript, a primer extension assay was carried out with K5R4 dye primer (Fig. 5).One product was situated 141 bp upstream of the initiation codon,with a splice occurring at the 5' noncoding region; a typicalsplice donor-acceptor site (GT...AG) was present in the intron ofthe K5 locus (Fig. 5); there was a putative CCAT box-like sequenceat a position 126 to 129 bp upstream of the initiation site; butno obvious TATA box-like sequence was found within 1.0 kb upstreamof the starting codon using the transcription factor database(32).

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FIG. 5. Map showing the K5 transcription pattern. (A) Schematic representation of the primer used in the primer extension assay and summary of the maps obtained using primer extension and 5' and 3' RACE. (B) Initiation site of the K5 transcript identified by primer extension. The size of the primer extension product is indicated by a sequencing ladder initiated with the same primer. The arrowhead indicates the position of the cDNA product, and the number indicates its position with respect to the initiation codon (ATG).

To determine the location of the 3' end of the K5 transcript, a 3' RACE assay was performed and only a single product wasgenerated. Sequencing showed the 3' end to be situated 24 nucleotidesdownstream of the putative poly(A) signal (Fig. 6).

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FIG. 6. Map of the K5 ORF. A putative CCAT box and the poly(A) signal are boxed and in boldface; note that they lack a distinguishable TATA box. The asterisk indicates the initiation site of the K5 transcript. The nucleotide sequence corresponding to the intron is boxed and shaded. The splice donor (GT...) and splice acceptor (...AG) sites are in boldface. The primers (K5F, K5F1, K5R1, K5R2, and K5R3) used for 3' and 5' RACE and RT-PCR are underlined. The arrows indicate the orientations of the primers.

K5 is expressed as an IE protein. The time course of K5 gene expression was determined using antigen plates prepared after selected periods of TPA treatment.BC-3 cells were used in this experiment instead of BCBL-1 cellsbecause less than 1% of uninduced BC-3 cells expressed the K5protein (Fig. 7a). This provided a lower background against whichto detect increases in K5 expression than would be obtained withBCBL-1 cells (4 to 5%; Fig. 1a). We found that approximately 20%of BC-3 cells were K5 positive after 4 h of TPA induction (Fig.7c) and that number increased to a maximum (80%) within 12 h afterinduction (Fig. 7f). By contrast, the K9 gene product, which isan early gene product (19), was first expressed 12 h after treatment(data not shown).

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FIG. 7. Fluorescence (FITC) photomicrographs showing the time course of K5 protein expression. BC-3 cells were left uninduced or induced with TPA. After 2, 4, 6, 8, and 12 h of induction, cells were labeled with MAb 328C7.

Northern blot analysis of total RNA extracted from BCBL-1 cells carried out using an ORF K5-specific probe showed a singletranscript of approximately 1.2 kb (Fig. 8A, lane 2). The sametranscript was clearly detected in cells treated with TPA plusPFA for 12 h (Fig. 8A, lane 6), indicating its independence ofviral DNA synthesis, and in cells treated with TPA plus CHX at10 µg/ml (Fig. 8A, lanes 5), although the transcript was barelydetectable in cells exposed to CHX at 33 µg/ml (Fig. 8A, lane4). Diminished $beta$ -actin in the presence of either CHX concentrationwas indicative of inhibited protein synthesis. On the other hand,K9, which is supposed to be an E gene, was repressed in the presenceof CHX at any concentration. This result confirmed that K5 wasone of the IE genes.

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FIG. 8. (A) Northern blot analysis demonstrating the resistance of K5 transcription to the presence of inhibitors of DNA and protein synthesis (PFA and CHX, respectively). Total cellular RNA was prepared from TPA-stimulated BCBL-1 cells after 12 h of exposure to PFA and CHX, size fractionated on a 1% agarose-formaldehyde gel, transferred to nylon membrane, and probed with K5- and K9-specific antisense DNA probes. From top to bottom, the autoradiograms shown are of blots hybridized with probes for the K5, K9, and $beta$ -actin (used as a loading control) genes, respectively. (B) Immunoprecipitation of K5 protein expressed in BCBL-1 cells following metabolic labeling with PFA and CHX. For detection of HHV-8 IE and E proteins, cells were induced with TPA and incubated for 12 h with PFA at 300 µg/ml. For detection of HHV-8 IE genes, cells were induced with TPA and incubated for 4 h with CHX at 100 µg/ml and then for 6 h with AcD at 10 µg/ml. Labeling with [³⁵S]methionine was performed 1 h before cells were harvested. Lysates were prepared and immunoprecipitated with MAb 328C7. Samples were separated by SDS-10% denaturing PAGE. Molecular mass markers are shown on the left (lane 1). The position of the 36-kDa protein is indicated. Samples in lanes 2, 3, 4, 5, and 6 are TPA treated, TPA-PFA treated, untreated, CHX treated, and CHX-AcD treated, respectively.

Immunoprecipitation assays yielded a 36-kDa band in samples treated with TPA alone or with TPA plus PFA (Fig. 8B, lanes 2and 3). No K5 protein expression was detected in cells treatedwith CHX (Fig. 8B, lane 5), but replacement of CHX with AcD restoredexpression of the 36-kDa protein. Thus, synthesis of the K5 geneproduct is independent of de novo viral gene expression and proteinsynthesis, which is consistent with its being an IE gene product.In addition, a second prominent band was observed at 70 kDa (Fig.8B, lane 6). Although its origin is unknown, this band may indicatethat under some conditions, the K5 protein exists as adimer.

Transregulation of the K5 gene. Because the majority of IE genes exert a regulatory effect on E and L gene expression, transregulation of the K5 gene wasexamined in two types of experiment. In the first, the responsivenessof the K5 gene promoter was assessed in cells transiently cotransfectedwith expression vectors pcDNA3-K5 and pcDNA3-KSHV/Rta and withreporter plasmid pk5-Luc. After 24 h of transfection, the cellswere collected by trypsinization, washed twice with PBS, and assayedfor luciferase activity. As shown in Fig. 9, luciferase activitywas increased about fivefold when pcDNA3-KSHV/Rta was cotransfectedwith pk5-Luc. In contrast, when pcDNA3-K5 and pk5-Luc were cotransfected,there was no significant stimulation of luciferase activity comparedwith cotransfection of an empty vector. In a second experiment,the transregulatory effect of K5 on homologous and heterologouspromoters of the HHV-8 polymerase (p8pol-Luc) and the HIV-1 LTR(pLTR-Luc) was tested and in neither case did K5 affect luciferaseactivity driven by these promoters (data not shown).

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FIG. 9. Responsiveness of the K5 gene promoter to the K5 gene and KSHV Rta. Transfected cells were harvested 24 h after transfection, and luciferase activity was assayed. Shown are the means ± standard deviations of triplicate transfections.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The HHV-8 K5 gene is a homologue of BHV-4 IE-1. BHV-4 possesses two IE genes, IE-1 and IE-2 (43), the latter being a homologueof EBV R and HVS R which acts as a transactivator and interactswith other proteins (44, 45). On the other hand, BHV-4 IE-1has no homology with the EBV genome; rather, it is a positionalhomologue of HVS gene 14 (9). Its putative product containsa cysteine-rich region that may form zinc fingers characteristicof some DNA-binding proteins (44), but no function has yet beenascribed to BHV-4 IE-1.

Using Western blots probed with an anti-K5 MAb, we identified a 36-kDa polypeptide in BCBL-1 (Fig. 3) and BC-3 cells infectedwith HHV-8, but not in those infected with EBV, and cDNA screeningshowed the protein to be encoded by ORF K5. This finding was confirmedby the ability of MAb 328C7 to react with a eukaryotically expressedfusion protein containing ORF K5 (Fig. 1e). Both cell types werestrongly positive for virus-specific antigen only after inductionwith TPA, suggesting that the K5 gene was not expressed duringthe latent stage of infection but was reactivated as part of acascade leading to replication. The low level of expression observedin uninduced cells (Fig. 1 and 7) probably indicates that a certainamount of spontaneous virus replication occurs in BCBL-1 and BC-3cells, as is seen in some cell lines harboring EBV (6, 25).

K5 protein synthesis in the presence of PFA, CHX, and AcD $---$ DNA, protein, and mRNA synthesis inhibitors, respectively $---$ indicatesthe independence of K5 gene expression from de novo viral proteinsynthesis, confirming its IE nature. Indeed, IE genes are knownto code for regulatory proteins and are expressed by host celltranscription and translation systems prior to viral DNA replication.Other HHV-8 IE and E gene candidates have been reported basedon levels of mRNA expression in BCBL-1 and BC-1 cells (23, 40,41, 46), but the method of their analysis was different fromours. They investigated the mRNA expression level using BCBL-1and BC-1 cells. K5 protein was detected as early as 4 h afterTPA induction in BCBL-1 and BC-3 cells, and expression was maximalwithin 12 h. In contrast, when BC-1 cells were induced with TPAand reacted with MAb 328C7, antigen expression was not detecteduntil 12 h after induction (data not shown). The reason for thedelayed expression in BC-1 cells is unclear, but the presenceof EBV in BC-1 cells may inhibit expression of the K5 gene. Therefore,to our knowledge, this is the first account of an HHV-8 IE geneproduct.

The K5 antigen was present in the cytoplasm $---$ particularly the ER $---$ of both HHV-8-infected cells and ORF K5 transfectants (Fig.1 and 2) but was absent from the virion and from the nucleus.Almost all other known herpesvirus IE antigens are found in thenucleus and are involved in regulation of the expression of othergenes (e.g., E and L genes). One exception is the varicella-zostervirus IE-4 antigen, which, like K5, is localized in the cytoplasm(10, 11). On the other hand, the varicella-zoster virus IE-4antigen has transactivational activity toward homologous and heterologouspromoters (10, 11) and during very early stages of infection,it is detectable in the nucleus (11). We observed no apparenttransactivational activity toward homologous and heterologouspromoters on the part of K5; nevertheless, by analogy, K5 mayexert a regulatory effect on gene expression at times earlierthan those at which we were first able to detect the protein inthe presentstudy.

Recently, KSHV Rta was shown to encode an IE gene that acts as a transactivator (23, 40). KSHV Rta is a homolog of EBVRta; its mRNA is partially resistant to treatment with CHX (40,41); and it transactivates the K5 promoter (Fig. 9). As theK5 protein did not transregulate its own promoter or a promoterdriving the expression of DNA polymerase or the HIV-1 LTR, itappears that K5 expression occurs downstream of KSHV Rta expression.Further analysis is required to more precisely evaluate the activityof K5 at very early times and to gain a more complete understandingof the biological function ofK5.

	ACKNOWLEDGMENT

This study was supported in part by a Grant-in-Aid from the Ministry of Education, Science and Culture ofJapan.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbiology, Osaka University Medical School, 2-2 Yamada-oka, Suita,Osaka 565-0871, Japan. Phone: 81-6-6879-3321. Fax: 81-6-6879-3329.E-mail: yamanisi{at}micro.med.osaka-u.ac.jp.

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Top
Abstract
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Materials and Methods
Results
Discussion
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