In Vivo Protein Binding and Functional Analysis of cis-Acting Elements in the U3 Region of the Bovine Leukemia Virus Long Terminal Repeat

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 Xiao, J.
	Articles by Buehring, G. C.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Xiao, J.
	Articles by Buehring, G. C.

Previous Article | Next Article

J Virol, July 1998, p. 5994-6003, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

In Vivo Protein Binding and Functional Analysis of cis-Acting Elements in the U3 Region of the Bovine Leukemia Virus Long Terminal Repeat

Jianqiao Xiao and Gertrude C. Buehring^*

School of Public Health, University of California, Berkeley, California 94720

Received 27 May 1997/Accepted 9 April 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Bovine leukemia virus (BLV) is a member of the human T-cell leukemia virus (HTLV)/BLV group of retroviruses. These virusesregulate their own transcription by producing Tax, a protein whichactivates the virus promoter region, the long terminal repeat(LTR). To explore the molecular mechanisms involved in the transactivation,we identified protein binding elements by in vivo footprintingand analyzed their function by site- directed mutagenesis. Weused in vivo dimethyl sulfate footprinting by ligation-mediatedPCR to detect constitutive in vivo protein-DNA interactions ina BLV-producing cell line, Bat₂Cl₆. The U3 region and part ofthe R region of the LTR were footprinted. In addition to the cis-actingelements (three cyclic AMP-responsive elements [CREs] and twoAP4 sites) reported by others to be important for Tax-mediatedactivation of the BLV LTR, we found footprints in regions flankingthese elements and in the core promoter region. The importanceof these sites for transcriptional activation was studied by site-directedmutagenesis followed by promoter function analysis of the mutantswith a chloramphenicol acetyltransferase reporter system. Ourdata corroborate those of others showing that the CREs are necessaryfor transactivation of the LTR, and they identify two new functionalsites not previously reported by others. We show that the middleregion of the BLV U3 contains multiple dual-functioning cis-actingelements which act as either positive or negative regulatory elementsdepending on the cell type tested. This is the first report ofa functional mapping of the cis-acting elements of a virus ofthe HTLV/BLV group.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Bovine leukemia virus (BLV) is the etiologic agent of enzootic bovine leukosis, a disease characterized by persistent lymphocytosisand development of B-cell lymphomas after a long latent period.It also causes chronic lymphocytic leukemia and lymphomas in experimentalanimals such as sheep and goats (reviewed in reference 24).BLV is a retrovirus closely related to human T-cell leukemia viruses(HTLV-1 and HTLV-2). Like HTLV, BLV contains a pX region betweenthe env gene and its 3' long terminal repeat (LTR), in additionto three genes common to all retroviruses: gag (group-specificantigen), pol (polymerase, endonuclease, and integrase) and env(envelope proteins). One of the proteins encoded in the pX regionis p34 Tax (transactivator from the X region), which acts on the5' LTR to stimulate transcription of the BLV genome (9, 10,25, 44). p34Tax can also activate some cellular promoterssuch as c-fos promoter (23). Expression of BLV in vivo is believedto be regulated by cellular trans-acting factors that bind tothe cis-acting elements in the U3 region of the BLV LTR in thepresence of p34 Tax (reviewed in reference 24).

The LTR region of a retrovirus consists of U3, R, and U5 regions. Although the R and U5 regions are essential for virus replication,it is the U3 region that is critical for transcriptional controlof a retrovirus (8). As with HTLV, the BLV U3 region containsthree imperfect direct repeats (DRs) of 21 bp (DR1, bp $-$ 163 to $-$ 143; DR2, bp $-$ 138 to $-$ 118; DR3, bp $-$ 63 to $-$ 43), which are calledtax-responsive elements (TREs) (9, 25, 44). In the middleof each 21-bp repeat is an octamer homologous to the core sequenceof the cyclic AMP-response element (CRE), each with only a 1-bpdifference from the consensus CRE sequence (Fig. 1). By analyzingthe promoter function of deletion mutants, Derse (9) and Katohet al. (23) found that the three CREs are cis-acting elementsimportant for the responsiveness of the BLV LTR to p34Tax. A fewother elements which may also be important in transcription regulationhave been identified: an E-box sequence (CAGCTG), which is thebinding site for the cellular transcription factor AP4 (the upstreamAP4 site [ $-$ 151 to $-$ 146] is hereafter designated AP4-1, and thedownstream one [ $-$ 124 to $-$ 119] is designated AP4-2) (42); a nuclearfactor $kappa$ B (NF- $kappa$ B) binding site (6); and a glucocorticoid responseelement (GRE) (29, 45a) (Fig. 1).

View larger version (22K):
[in this window]
[in a new window]

FIG. 1. cis-acting elements in the U3 region of BLV. (A) Schematic map of the BLV LTR showing the locations of the cis-acting elements in the U3 region and the binding sites for the primers used for in vivo footprinting. (B) Nucleotide sequence comparison of response elements in the BLV U3 region: the TREs, consensus CRE and CRE-like sequences including the AP4 sites, and the consensus GRE and GRE-like sequence. Bases different from the consensus sequences are shown in boldface type.

Although p34Tax does not bind DNA directly (1, 44), it has been shown, by in vitro studies of others, to interact directlywith the proteins binding to some of the cis-acting sequences,e.g., members of the CREB/ATF family of bZip proteins which wereshown to bind the CRE-like sequences in vitro (4, 25). p34Taxmay also interact with other cellular transcription factors thatrecognize some of these sequences, such as AP4 and NF- $kappa$ B (6,42). For HTLV, it was shown that transactivation of the LTRinvolves interactions between p40Tax and multiple cellular transcriptionfactors (reviewed in reference 1). Transcription factor CREBfunctions as either a positive or negative regulator dependingon whether it binds to the CRE-like sequences in the U3 regionor to a nonconsensus CRE sequence in the R region (46). It hasbeen reported that both positive and negative regulatory elementsare present in the LTR region of other retroviruses such as humanimmunodeficiency virus, mouse mammary tumor virus, and Rous sarcomavirus, and that cellular regulatory factors that bind to specificsequences in the LTR region of these viruses are responsible forthe regulation of viral expression and tissue specificity of theseviruses (5, 18, 21, 40, 47).

BLV is usually nondetectable in vivo in infected lymphocytes or tumor cells (reviewed in reference 24), but nothing is knownabout how BLV expression is suppressed in vivo. It is obviousthat interactions between p34Tax and cellular proteins activatethe viral promoter, but whether similar interactions are involvedin repressing transcription has not been studied. We sought toclarify these interactions by determining the sites in the U3region of the BLV at which LTR proteins are bound and whetherthese proteins function cooperatively with BLV p34Tax to controlthe expression of BLV by binding to negative regulatory elements(NREs) and/or positive regulatory elements (PREs). First we lookedat constitutive in vivo protein-DNA interactions in the U3 regionin a virus-producing cell line, Bat₂Cl₆. Then we applied site-directedmutagenesis to delete or mutate the individual protein-bindingsites we detected (13 of the protein-binding sites and 1 sitewith no visible footprints were mutated or deleted, and 25 mutantswere created). The wild-type and mutant LTRs were cloned intochloramphenicol acetyltransferase (CAT) reporter constructs, andpromoter function was analyzed in six cell lines, representingdifferent species and tissue types, by transient gene transfectionassays in the presence or absence of Tax.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cell lines. Tb₁Lu, a bat lung epithelial cell line negative for BLV (16), was from the University of California San Francisco Cell CultureFacility (San Francisco, Calif.). Bat₂Cl₆, a BLV-producing cellline derived from Tb₁Lu cells infected with the virus by cocultivationwith lymphocytes from a BLV-infected cow (16), was obtainedfrom K. Radke (University of California Davis, Davis, Calif.).FLK, a BLV-producing fetal lamb kidney fibroblast line (43),and MCF-7, a mammary epithelial cell line established from a humanbreast carcinoma (38), were obtained from the former Naval BiosciencesLaboratory (Oakland, Calif.). GR, a cell line derived from a mousemammary tumor (26), was obtained from G. Firestone (Universityof California Berkeley, Berkeley, Calif.). Raji, a human B-cellline derived from a Burkitt's lymphoma (12, 32), was obtainedfrom R. Emmons (California Department of Health Services, Berkeley,Calif.). BL3, a BLV-infected bovine B-lymphocyte line, was obtainedfrom Harris Lewin (University of Illinois, Champaign, Ill.). Celllines were maintained in Dulbecco's modified Eagle's medium (DMEM)(GIBCO, Grand Island, N.Y.) or, for BL3, Liebovitz medium (GIBCO)supplemented with 5 to 10% heat-inactivated fetal bovine serum(FBS) (Sigma, St. Louis, Mo.), 10 µg of insulin (Sigma) per ml,and antimicrobial agents and incubated at 37°C in a humidifiedatmosphere of 5% CO₂.

In vivo footprinting with DMS. (i) Primers and linkers used for footprinting. The primers and linkers used are described in Table 1 and are based on the BLV provirus sequence reported by Sagata et al.(35). Oligonucleotides were synthesized either by the MicrochemicalFacility, Department of Molecular and Cell Biology, Universityof California, Berkeley, or by Operon Biotechnologies, Alameda,Calif. A common linker was prepared by annealing equimolar amountsof each linker in 250 mM Tris-HCl by the method of Pfeifer andRiggs (31).

View this table:
[in this window]
[in a new window]

TABLE 1. Sequences of primers and linkers used in this study

(ii) DNA preparation, primer extension, and ligation. DNA preparation, primer extension, and ligation were done by the method of Pfeifer and Riggs (31). Briefly, DNA was extractedby standard phenol-chloroform procedures (36) from Bat₂Cl₆ cellswith or without DMS treatment. DNA from cells not treated withDMS was treated with DMS after purification. DNA methylated withDMS was then cut with hot piperidine (90°C), precipitated, dried,and redissolved in distilled water at 0.5 to 1.0 µg/µl. Primerextension and ligation were done exactly as described by Pfeiferand Riggs (31) with 1 µg of each cleaved template for each reaction.Primers A1, B1, and C1 (Table 1) were used for primer extensionto make double-stranded DNA fragments, which were ligated to thecommon linker (prepared by annealing linkers 1 and 2) (Table 1).

(iii) PCR. A two-round PCR was used to amplify the U3 region of BLV provirus DNA (from Bat₂Cl₆ cells) in a thermal cycler (Perkin-ElmerCetus, Norwalk, Conn.). Ligated DNA (50 µl) was mixed with 50µl of freshly made 2× PCR reaction mix (10 µl of 10× Taq polymerasebuffer [Mg²⁺ free; Promega, Madison, Wis.]; 10 µl of 25 mM MgCl₂; 1 µl each[20 pmol] of primer A2, B2, or C2; 1 µl [20 pmol] of linker 1;0.8 µl of 10 mM deoxynucleoside triphosphates [dNTPs; Promega],3 U of Taq polymerase; 27 µl of water). The reaction mix was heatedto 95°C for 5 min to denature the DNA and then run with the followingcycle profile: 94°C for 1 min, 60°C for 2 min, and 75°C for 3min for 35 cycles. To extend all DNA fragments completely, anadditional incubation at 72°C was done for 20 min. The PCR productswere extracted by the standard phenol-chloroform procedure, precipitated,dried, and dissolved in 20 µl of distilled water. The second-roundPCR was run in a 10-µl volume containing 1× Taq polymerase buffer(Promega), 2 µl of the PCR-amplified DNA (see above), 0.5 U ofTaq polymerase, 2.5 mM MgCl₂, 200 µM each dNTP, and about 100fmol (25,000 cpm) of primer A3, B3, or C3, which was 5'-end labeledwith ³²P by using T4 DNA kinase (Promega) and [ $gamma$ -³²P]ATP (Amersham, Arlington Heights, Ill.) and gel purified bystandard methods (36). The samples were heated at 95°C for 2.5min, and then 25 to 30 cycles of 95°C for 30 s, 66°C for 1 min,and 75°C for 2 min were run with a 20-min incubation at 72°C atthe end. A 5-µl volume of stop buffer (95% formamide, 1 mM EDTA,0.5% xylene cyanol, 0.5% bromphenol blue) was then added to eachreaction mixture. The PCR products were analyzed by a 6% polyacrylamide-ureasequencing gel run as suggested by the manufacturer (Bio-Rad Laboratories,Hercules, Calif.). The DNA concentration of the samples was standardizedby loading equal counts per minute. After electrophoresis, thegel was dried and exposed to Fuji X-ray film for 12 to 96 h. Thefilm was developed manually.

Site-directed mutagenesis of the BLV LTR. (i) Preparation of plasmid DNA. The pGEM-T plasmid used to clone the BLV LTR was purchased from Promega. pBL CAT3 plasmid, which contains only the basic chloramphenicolacetyltransferase (CAT) gene without any eukaryotic promoter (27),was kindly provided by Isabelle Cludts. Escherichia coli TG1 cellswere transformed with the appropriate plasmid as described bySambrook et al. (36). Large-scale plasmid DNA was prepared asdescribed by Sambrook et al. (36) by the alkali lysis and CsCl-ethidiumbromide banding methods. Plasmid minipreps were prepared by QiagenQuick Spin plasmid purification kits as specified by the manufacturer.

(ii) DNA sequencing. DNA sequencing was done with the Silver Sequence DNA-sequencing system (Promega), which uses the enzymatic method of Sangeret al. (37). The sequencing reaction was done in a thermal cycler(Perkin-Elmer Cetus). The sequencing gel was stained with silvernitrate, and permanent records were made by exposing the gel (for10 to 15 s) to Silver Sequence film (Promega), which was developedmanually.

(iii) Restriction enzyme digestion and ligation reaction. All the restriction enzymes and T4 DNA ligase were purchased from Promega. For restriction enzyme digestion, 1 to 20 µg ofplasmid DNA was digested at 37°C for 2 h to overnight in the bufferprovided by the manufacturer. DNA fragments of interest were purifiedwith a GeneClean kit (Bio 101, La Jolla, Calif.). All the ligationreactions were performed as described by Sambrook et al. (36).Briefly, 50 to 100 ng of each vector and insert DNA (equimolar)was mixed with 0.2 U of T4 DNA ligase in 10 µl of 1× ligationbuffer (20 mM Tris HCl [pH 7.7], 5 mM MgCl₂, 5 mM dithiothreitol,1 mM ATP) and incubated at 16°C for 3 h. Then 1 to 2 µl of theligation mix was used to transform competent TG1 cells as describedabove.

(iv) Construction of CAT plasmids. Construction of CAT plasmids was generally done by standard procedures (36). The whole LTR region of BLV was amplified byPCR with Bat₂Cl₆ DNA as the template and BLV LTR specific oligonucleotidesas primers (Table 1). The LTR PCR product was first cloned intothe pGEM-T vector (Promega) in the 5'-to-3' direction (confirmedby sequencing) as specified by the manufacturer. The LTR DNA wasthen subcloned into plasmid pBL CAT3 upstream of the CAT gene.Clones containing inserts (which have a higher molecular weightthan the parental plasmid) were selected, and the cloned DNA wasfurther amplified in TG1 cells. The orientations of the LTR insertswere determined by restriction enzyme digestion, and the U3 regionof BLV LTR in the constructs was sequenced to confirm that thesequence was correct. The same method was used to construct mutantLTR-CAT plasmids after the mutations were made in plasmid pGEM-T/LTR(described below).

(v) PCR amplification. The reaction was done in 50 µl of 1× PCR buffer (10 mMTris-HCl [pH 8.3], 50 mM KCl, 2 mM MgCl₂, 5 mM 2-mercaptoethanol, 0.005%gelatin) containing 10 pmol of each primer, 100 to 500 ng of templateDNA, 2.5 U of Taq polymerase, and 0.2 mM each dNTP. The reactionwas performed in a thermal cycler with the following cycling profile:94°C for 1 min, 50 to 56°C for 1 min, and 72°C for 2 min for 30cycles followed by an extension cycle at 72°C for 10 min. ThePCR products were stored at $-$ 20°C until use.

(vi) Mutagenesis of cloned BLV LTR. The method of Rashtchian et al. (33) was modified to create mutations or deletions in the cloned BLV LTR. Vector and universalprimers used for mutagenesis are listed in Table 1. In addition,one pair of mutagenic primers was synthesized for each mutantto introduce a small deletion or base substitution. Mutagenicprimers are not included in Table 1, but the mutations introducedare summarized in Table 2. Each mutagenic primer was 20 baseslong and corresponded to the wild-type LTR sequence except forthe introduced mutation approximately in the center of the sequence.Three PCRs were run separately with three pairs of primers: vectorprimers were used to amplify most of the pGEMT vector DNA (bp1000 to 3000), universal primer 1 coupled with a mutagenic primer1, and universal primer 2 with a mutagenic primer 2 were usedto amplify part of the plasmid and part of the cloned LTR. ThreePCRs amplified the complete sequence of the vector containingthe cloned LTR. Since the universal primers overlapped the vectorprimers, since mutagenic primer 1 overlapped mutagenic primer2, and since the thymidines in the overlapping region were replacedby uridines, amplification of the template plasmid by PCR resultedin the incorporation of the primers and the desired mutation intothe PCR products. Excision of the deoxyuracil residues in thePCR products by uracil deoxynucleotide glycosylase (UDG) destabilizedbase pairing at the ends of DNA molecules and thus generated 3'protruding ends. Due to the overlapping nature of the primers,the resulting 3' protruding ends were complementary and couldanneal after treatment with UDG.

View this table:
[in this window]
[in a new window]

TABLE 2. Sequence changes of 25 BLV LTR mutants made by site-directed mutagenesis

After the PCRs, 5- to 10-µl volumes of each of the three PCR products were combined and 1 U of UDG was added to the mixture,which was then incubated at 37°C for 30 min, heated at 98°C for15 min to cleave the abasic nucleotides, and reincubated at 37°Cfor 30 min (annealing). The UDG-treated PCR products were thenethanol precipitated and dissolved in 5 to 10 µl of water. A 2-µlvolume of this DNA solution was used to transform competent TG1cells. The template DNA was treated so that no intact circularplasmid DNA was left; i.e., no transforming colony could be foundafter transforming the cells by using the PCR products withoutUDG treatment. Only the mutant plasmid DNA formed by annealingof the UDG-treated PCR DNA could transform the bacteria. For reactionswith universal and mutagenic primers, the plasmid was linearizedwith SspI, which cuts the vector three times at positions 2199,2384, and 2408. For reaction with the vector primer, the templatewas treated with SacI and SacII, which cut the vector at bp 94and 46, respectively. Miniprep plasmid DNA was prepared from thetransformed colonies, and sequencing analysis was done to screenthe mutants containing the desired sequence changes.

Gene transfer. Tb₁Lu cells were used to detect the promoter function of the BLV LTRs (wild type and mutants) which were cloned upstream ofthe CAT gene. For each transfection, 4 × 10⁵ to 5 × 10⁵ cells were seeded into a 35-mm petri dish and cultured for 24h, and then the cells were transfected with plasmid DNA by usingLipofectamine (GIBCO) as specified by protocol provided by themanufacturer. Serum-free DMEM was the transfection medium, and6 µl of Lipofectamine was used. Cells were incubated with theDNA-Lipofectamine mixture for 20 h before DMEM with FBS was addedto a final concentration of 10% FBS. The cells (~10⁶/dish) were harvested for CAT assay 48 h after the transfectionwas started. To detect basal promoter function, 1 µg of LTR-CATplasmid DNA was used for each 35-mm dish. To detect promoter functionin response to p34Tax, 0.5 µg of each LTR CAT DNA and 0.5 µg ofpSG-tax plasmid DNA (a kind gift from Luc Willems), which containsthe BLV tax gene under the control of the simian virus 40 earlypromoter, were used for each 35-mm plate.

CAT ELISA. The promoter function of the BLV LTR was measured as the amount of CAT protein produced by the transfected cells. CAT wasdetected by an enzyme-linked immunosorbent assay (ELISA) withthe CAT ELISA kit (Boehringer-Mannheim, Indianapolis, Ind.) asspecified by the manufacturer. Briefly, 48 h after transfection,cells were lysed with 0.5 to 1 ml of kit lysis buffer. Cell lysateswere pelleted, and 50 to 100 µl of the supernatant was used forthe ELISA. The absorbance readings were translated into CAT proteinconcentrations from a standard curve established simultaneouslyin each ELISA experiment, and the amount of CAT protein in eachsample was adjusted according to the concentration of total proteinsin the cell lysate. The protein concentration was measured withthe bicinchoninic protein assay system as specified by the manufacturer(Pierce, Rockford, Ill.).

EMSA. Oligonucleotides representing wild-type or mutated protein binding sites were used as probes (Table 1). Double-stranded oligonucleotideswere obtained by mixing the complementary strands in a 1:1 ratio,heating to 80°C for 5 min, and cooling at room temperature for1 h to anneal; they were stored at 4°C. For each electrophoreticmobility shift assay (EMSA) experiment, 1 pmol of each oligonucleotidewas 5'-end labeled with [ $gamma$ -³²P]ATP (Amersham) and gel purified (36). Nuclear protein extractswere prepared from Bat₂Cl₆ and Tb₁Lu cells essentially as describedby Adam et al. (1). Extracts were stored at $-$ 70°C until use.

A 1-µl volume of cell extract ( $approx$ 2 µg of total protein) was mixed with 1 µg of sheared calf thymus DNA and 5 µl of ³²P-labeled oligonucleotide probe (10 fmol; 30,000 cpm) in 13 µlof binding buffer (40 mM NaCl, 20 mM Tris-HCl [pH 7.5], 4 mM DTT,1 mM EDTA, 0.002% Triton X-100, 750 µg of bovine serum albuminper ml, 10% glycerol). The mixture was incubated for 1 h at roomtemperature and then separated on a 5% polyacrylamide gel (10V/cm) in 90 mM Tris-borate buffer with 2 mM EDTA. The gels weredried and subjected to autoradiography at $-$ 70°C with intensifyingscreens.

Statistical analysis. For CAT assays, differences between the various mutants and the wild type were analyzed by the Dunnett t test. This is a multiple-comparisonmethod which uses a pooled standard deviation and allows a comparisonof multiple values to a single control. The minimum significancelevel was P < 0.05 (two-sided test).

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

In vivo footprinting reveals multiple protein-binding sites in the U3 region of BLV. Figure 2 shows the DMS methylation patterns of both the noncoding strand (lanes 1 and 2, primer set A) and the coding strand(lanes 3 and 4, primer sets B and C) of the U3 region of BLV.At three CRE sites, two AP4 sites, the TATA box, and the putativeGRE site, the guanidines were protected from DMS methylation onat least one strand, suggesting that these areas are protein bindingsites. In the NF- $kappa$ B site (bp $-$ 70 to $-$ 118), which contains a CATbox in the middle, the guanidines were protected at several siteson both strands, but one hypersensitive sites (bp $-$ 106 to $-$ 107)was found on the noncoding strand. This suggests that the NF- $kappa$ Bsite is bound by multiple proteins or a large protein complex.In addition, protein contacts were found in sequences on bothsides of the DR1/DR2 region, in the core promoter region (bp $-$ 40to +1), and in the R region shown on this gel (from RNA startsite to bp +30) and showed decreased sensitivity to DMS for mostof the residues, with a few hypersensitive ones.

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

FIG. 2. In vivo DMS footprinting of the BLV U3 region in the presence of Tax. BLV-infected Bat₂Cl₆ cells were used as the source of DNA. Lanes: 1 and 2, noncoding strand with primer set A; 3 and 4, coding strand with primer sets B and C. In vitro (purified DNA) DMS-treated samples are in lanes 1 and 3. In vivo (living cells) DMS-treated samples are in lanes 2 and 4. The locations of the bands relative to the RNA start site are labeled at the left of each gel (negative numbers for sequences upstream and positive numbers for the downstream of the start site). Increased sensitivity to DMS (band in lane 2 darker than in lane 1, and band in lane 4 darker than in lane 3) is indicated by arrows pointing away from the gel, and decreased sensitivity to DMS (lighter or no bands in lanes 2 and 4) is indicated by arrows pointing toward the gel. cis-acting elements reported in the literature are indicated by open boxes on the right of the gel, the consensus sequences of the AP4 sites are indicated by solid boxes, the core sequences of three CRE-like elements are indicated by the hatched boxes, and the GREs are indicated by dotted boxes.

Site-directed mutagenesis, EMSA (gel shift), and transient gene transfection studies were used to further evaluate the invivo protein binding sites. The sequences of 13 protein bindingsites and 1 site with no detectable protein contacts were mutatedby site-specific mutagenesis, resulting in a total of 25 mutants(Table 2). Sequences of these mutants were confirmed by sequencingboth before and after subcloning into pBLCAT3 plasmid (data notshown). The promoter function of these mutant LTRs was determinedby a CAT ELISA after the plasmid DNA was transfected into Tb₁Lucells (a cell line identical to Bat₂Cl₆, except that it is notinfected with BLV). The basal promoter activity of the wild-typeand mutant LTRs (in the absence of p34Tax) was detected by transfectingTb₁Lu cells only with the LTR-CAT plasmid. To determine the functionof the wild-type or a mutant LTR in response to p34Tax, we cotransfectedthe LTR-CAT plasmid DNA into Tb₁Lu cells with plasmid pSGtax,which contains the BLV tax gene driven by the simian virus 40early promoter.

Mutations in protein binding sites decrease or abolish protein binding. Three of the protein binding sites detected by in vivo footprinting were further tested for protein binding by EMSAs. Figure3 shows that wild-type sequences corresponding to CRE2 and site $-$ 142 to $-$ 143 bound to nuclear proteins from BLV-producing Bat₂Cl₆cells but not from BLV-negative Tb₁Lu cells. In vitro proteinbinding at CRE2 was abolished by a 3-bp deletion; protein bindingat site $-$ 142 to $-$ 143 was diminished by a 2-bp substitution. Asreported in a separate communication, the putative GRE site demonstratedbinding to purified glucocorticoid receptor protein, and thisbinding was abrogated by each of six different types of mutations(45a).

View larger version (34K):
[in this window]
[in a new window]

FIG. 3. Gel shift assay to detect in vitro protein binding to wild-type and some mutant cis-acting elements in the BLV LTR. Synthetic double-stranded oligonucleotides were end labeled with [ $gamma$ -³²P]ATP and used as probes. Nuclear protein extracts were prepared from Bat₂Cl₆ (BLV-producing cell line) and Tb₁Lu (BLV-free parental cell line of Bat₂Cl₆). Labeled probes were incubated with nuclear extracts in the presence (+) or absence ( $-$ ) of unlabeled probe (100 times the concentration of the labeled probe) and separated on a 5% nondenaturing polyacrylamide gel. Protein-bound and free probes are indicated by the arrowheads. Tb₁Lu cell extracts were used for lanes 1, 4, 7, and 10 and Bat₂Cl₆ cell extracts were used for the remaining lanes.

Basal LTR promoter activity (in the absence of p34Tax) is abolished by any mutation at any of the protein binding sites. In the absence of p34Tax, all mutants except the negative control mutant (s-167) showed three- to sixfold lower activity thanthe wild-type LTR (Fig. 4A); the difference was statisticallysignificant by the Dunnett t test. The negative-control sequencewas from a site where no footprints were found; this mutant (s-167)was the only one to show a similar function to the wild-type LTRin both the absence and presence of p34Tax (Fig. 4A and B).

View larger version (37K):
[in this window]
[in a new window]

FIG. 4. Basal promoter function of the wild-type BLV U3 and 25 LTR mutants in the absence (A) and presence (B) of p34Tax (solid bars) with values in the absence of p34Tax (open bars) shown for comparison. LTRs were inserted into a CAT reporter construct and transfected into BLV-negative Tb₁Lu cells with or without cotransfection with a tax-containing plasmid. Mutants are arranged according to their location on the U3 map (Fig. 1). Promoter activity was measured as nanograms of CAT protein per 10 µg of total protein, and values were standardized by scaling the activity of the wild-type LTR to 1.0. Each value is the mean of five (A) or two (B) trials in separate experiments. Asterisks indicate that the CAT activity of the mutant is significantly different from the wild-type LTR (P $<=$ 0.05 [Dunnett t test]). Abbreviations: a, addition; d, deletion; s, substitution; WT, wild type. Acronyms in capital letters refer to sites illustrated in Fig. 1.

The LTR promoter activity of mutants in the presence of p34Tax is decreased, increased, or unchanged depending on the location of the mutated protein binding site. (i) Mutants with activity similar to the wild type. In addition to the negative control (s-167), six mutants showed activity similar to the wild-type LTR. These six involveddeletions or mutations in the DR1 region (s-AP4-1 and s-140),the DR3 region (d-CRE3, s-CRE3, and d-CRE3/aGRE), or both (d-CRE1/3)(Fig. 4B).

(ii) Mutants with decreased promoter activity. Seven mutants showed only 0 to 20% of the wild-type LTR promoter activity. Two of these mutants involved a mutation or deletionof a single protein binding site in the DR1 region (s-142-3 andd-CRE1) (Fig. 4B). The other five mutants all had deletions ormutations in two or all the CREs with or without mutations inthe GRE region.

(iii) Mutants with increased promoter activity. Eleven of the mutants had significantly stronger responsiveness to Tax than did the wild-type LTR (Fig. 4B; from left to right,d-CRE2, s- AP4-2, s-116, s-107,8, d-CRE1/2, s-99, s-83,4, s-GRE,d-CRE1/s-GRE, d-CRE2/s-GRE, and s,a-TATA). All these mutants involvesequence changes in the middle region of U3, including the DR2,GRE, CAT box, and its flanking sequences (NF- $kappa$ B site). Deletionin both CRE1 and CRE2 (d-CRE1/2) resulted in significantly higherCAT activity than that of the wild type. A 3-nucleotide deletionin CRE2 (Fig. 4B, d-CRE2) increased the promoter function threefold,and the mutant with both a deletion and a GRE mutation (d-CRE2/s-GRE)showed a further increase in promoter activity.

Of these 11 mutants, 3 contained only a single mutation (Table 2) (s-AP4-2, s-116, and s-99). It is interesting that a single-base-pairmutation in AP4-1 (Table 2, s-AP4-1) did not change the promoterfunction significantly but the same mutation in AP4-2 (s-AP4-2)gave rise to the strongest promoter function of all mutants, 14times that of the wild-type LTR. Point mutations at $-$ 116, (s-116), $-$ 107 to $-$ 108 (s-107,8), $-$ 99 (s-99), and $-$ 83 to $-$ 84 (s-83,4) increasedpromoter function three- to fivefold, respectively (Fig. 4B).The TATA box ( $-$ 43 to $-$ 36) was mutated so that it contained anAT-to-TA change at the beginning and a T addition at the 3' end(Table 2). This dramatically increased the CAT activity ( $approx$ 12-fold).

The effect of mutations on LTR promoter activity varies in different cell types. To examine the role of the host cell in the function of BLV cis-acting elements, we determined the CAT activity of 11 LTRmutants in five other cell lines besides Tb₁Lu: BL3, a BLV-infectedbovine B-lymphocyte cell line; Raji, a human B-lymphocyte cellline; FLK, a BLV-producing fibroblast cell line from fetal lambkidney; GR, a mouse mammary epithelial cell line; and MCF-7, ahuman mammary epithelial cell line. These cell lines were chosenbecause they originated from different cell types and speciesand also because they are convenient for transfection studies.The constructs used were the ones that contained a mutation ordeletion at only one protein binding site, so that the functionsof individual protein-binding sites could be analyzed. The effectsof mutations on promoter function are shown as increased or decreasedCAT activity of the mutants relative to the wild-type LTR. TheCAT activity of the LTR mutants in the six different cell linesis shown in Fig. 5. Three types of responses of the mutants top34Tax were found: (i) mutations at CRE1 and CRE3 are the onlyones that showed decreased CAT activity in all the cell lines(some decreases were not statistically significant); (ii) theCAT activity of some mutants was similar to that of the wild-typeLTR in some cell lines but increased or decreased in other celllines; and (iii) FLK and Tb₁Lu were the only cell lines to showany increased activity with mutations at any site.

View larger version (33K):
[in this window]
[in a new window]

FIG. 5. Promoter function of the wild-type BLV LTR and 11 LTR mutants in six different cell lines: BL3 (bovine B lymphocytes) (A), Raji (human B lymphocytes) (B), FLK (sheep fibroblasts) (C), GR (mouse mammary epithelial cells) (D), MCF-7 cells (human mammary epithelial cells) (E), and Tb₁Lu (bat lung epithelium) (F). For BL3 and FLK cells, only the plasmid with the wild-type or mutant LTR sequences was transfected, since these cell lines contain endogenous p34Tax. For the other four lines, wild-type or mutant LTR was cotransfected into cells with the pSGtax plasmid. Bars represent the mean values (nanograms of CAT protein per 10 µg of total protein) from two to four independent experiments. Values were standardized by scaling the activity of the wild-type LTR to 1.0. Asterisks represent statistically significant differences (P $<=$ 0.05 [Dunnett t test]) relative to the wild-type LTR.

The BLV U3 region of BLV can be largely divided into four functional units. Figure 6 summarizes the data from in vivo footprinting of the BLV U3 region in the virus-producing Bat₂Cl₆ cells and the CATassays to detect promoter function of the mutants in Tb₁Lu cells.According to CAT activities of mutant LTRs, the U3 region wasshown to contain four functional units: a core promoter region,from the RNA start site to the 5' of the TATA box; a dual regulatoryregion, from the 5' end of DR3 to the 5' end of AP4 (includingCRE2, AP4, the NF- $kappa$ B site, and GRE); and two positive regulatoryregions, CRE1 and DR3.

View larger version (34K):
[in this window]
[in a new window]

FIG. 6. Functional regions of the BLV U3. The genome structure of the whole BLV provirus is shown at the top. A schematic map of the U3 region is shown in the middle of the figure. The locations of three DRs are indicated by brackets. Possible protein binding sites are marked with boxes of different shapes (indicating different types of proteins). The locations of sequence changes in 15 mutants are indicated by asterisks (14 of the sites had altered in vivo footprints; no footprints were detected at bp $-$ 167). Mapping of the U3 region was based on the promoter activity of the mutants. Mutants with increased promoter activity were used to define an NRE, and the ones with decreased activity were used to define a PRE. The core promoter region was defined as reported in the literature (6, 9, 10). Regulatory regions were defined according to the reactions represented in Fig. 4B. Elements within the dually functional region function as NREs in some cell lines and as PREs in other cell lines.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Using in vivo footprinting and EMSA, we demonstrated multiple protein binding sites in the U3 region of the BLV LTR, and bysite-directed mutagenesis and transient gene transfection studies,we found that protein-DNA interactions at these sites are importantfor the transactivation of the BLV LTR. In the absence of p34Tax(Fig. 4A), all except one of the mutants showed lower CAT activitythan the wild-type LTR, indicating that basal promoter activityof the BLV LTR requires an intact U3 region in which none of theprotein binding elements are dispensable. The only mutant (s-167)that showed basal CAT activity similar to the wild-type LTR wasthe one at a position where no footprints were found (Fig. 2).It was used as a negative control. These results suggest thatbinding of cellular proteins to viral cis-acting elements is necessaryfor the basal-level promoter function of the LTR and may explainhow BLV transcription is launched in the initial absence of p34Tax.

In the presence of p34Tax, however, the promoter function of the mutants varied with each mutated protein binding site andwith the cell type used. Footprints were obvious at three CRE-likecis-acting elements shown by others to be recognized by cellularproteins in EMSAs (1, 44). Partial deletion of the core sequencesof CRE1 and CRE3 reduced the CAT activity in all cell lines tested(Fig. 5), suggesting that these elements may be the binding sitesfor ubiquitous positive regulatory proteins. Since CRE3 is immediatelyupstream of the TATA box, the transcription factor specific forthis element may help stabilize the binding of the TATA factor(TFIID) to the TATA box. Hirano and Wong (20) demonstrated thatsuch interaction is possible and that proteins binding to thepromoter containing the TATA box and the upstream enhancer elementsare cooperative in their function. This may explain why a deletionin CRE3 had a greater effect than the one in CRE1. The cooperativeeffects of the three CREs on the promoter function of BLV LTRwere studied in the Tb₁Lu line. Various mutants were made to containa deletion of 3 to 5 bp in one, two, or all three of the CRE coresequences. Our findings that CRE2 alone (when both CRE1 and CRE3were partially deleted) was able to maintain some normal functionand that the CRE2 sequence was able to be bound by proteins invitro (Fig. 3) are consistent with the results of previous studiesby Katoh et al. (23), who reported that a synthetic promotercontaining only CRE2 was responsive to BLV p34Tax. We found thatCRE1 had no function in the absence of intact downstream CREs,although it may function as an upstream enhancer in p34Tax-mediatedtransactivation of the BLV LTR (9). In our study, the mutantcontaining CRE3 alone (both CRE1 and CRE2 were partially deleted)had significantly increased function. In contrast, Derse (9)found that CRE3 was almost nonfunctional in the absence of theupstream cis-acting elements. In his study, large deletions createdby restriction enzymes, rather than small deletions made by site-directedmutagenesis, were used and all the sequences upstream of CRE3were deleted. These technical differences may explain the discrepantresults. Truncation of the upstream sequence may affect proteinbinding at downstream cis-acting elements close to the core promoter.Parekh and Hatfield (30) reported that proteins binding to anupstream activating sequence can activate transcription from adownstream promoter by DNA bending.

We found footprints at two AP4 sites shown by others to be recognized by proteins in gel shift assays (42) and in in vitro(DNase I) footprinting assays (6). Like Unk et al. (42),we found that transcription factor AP4 may be involved in thetransactivation of BLV LTR, but according to our data, the effectmay vary with the cell line and is affected by sequences flankingthe E-box, since the same point mutation in AP4-1 and AP4-2 affectedthe function of the LTR differently in different cell lines. Sincethe AP4 sites overlap those of the CREs, binding of AP4 to itsconsensus sequence may also be affected by other regulatory proteinssuch as CREBs. AP4 may either enhance or suppress the functionof the LTR depending on which of the two sites it binds.

Mutations in the NF- $kappa$ B site (Fig. 6; Table 2, s-83, 4, s-99, and s-116) also showed opposite effects in different cell types.Our finding are consistent with previous reports that the NF- $kappa$ Bsite is a dual-function element. In addition to functioning asa transcriptional enhancer element for a variety of genes (reviewedin reference 6), it can exert a negative effect on some cellulargenes (13-15). The negative effect of the NF- $kappa$ B site can also resultfrom binding of other repressors that compete with NF- $kappa$ B for theDNA sequence (15).

It is surprising that mutation of the TATA box also had different effects in different cell lines. Possible explanations comefrom previous observations that the function of the transcriptioninitiation complex is affected by the upstream enhancer bindingtranscription factors (17, 20, 22). Grayson et al. (17)also showed that subtle sequence changes in the TATA box affectedthe tissue-specific function of the myoglobin gene promoter. Itis likewise possible that the presence or absence of tissue-specifictranscriptional factors determines whether the BLV TATA box isfunctional.

Our data indicated that novel cis-acting elements other than CREs, AP4 and NF- $kappa$ B sites may play a role in the BLV LTR transactivation.One such element, as yet unnamed, is presumably located at the3' end of DR1, since a 2-base mutation at $-$ 142 and $-$ 143 significantlyreduced the promoter activity of the LTR (Fig. 4B, s-142,3, P< 0.005) and greatly reduced protein binding in the gel shiftassay (Fig. 3). Another such element is the GRE-like sequencejust upstream of the CRE3, which we have previously shown to bea key element in the responsiveness of BLV to glucocorticoidssuch as dexamethasone (29, 45a).

Both positive and negative regulation may be involved in the transcriptional activation of the BLV LTR. If a deletion or mutationresults in decreased activity, it indicates that the cis-actingelement is necessary for promoter activation and therefore isa PRE. On the other hand, if a deletion or mutation leads to increasedpromoter function, it suggests that this sequence is an NRE normallybound by a protein which suppresses the transcription activationof the LTR. In the presence of p34Tax, two AP4 sites, the second21-bp repeat (DR2), the NF- $kappa$ B site, and the GRE function as eitherPREs or NREs. However, in the absence of p34Tax, all sites functionas PREs. There are at least two possible explanations for this:(i) some cellular proteins may function as transcription factorsto maintain low-level transcriptional activity in the absenceof p34Tax, but they can function as repressors in the presenceof p34Tax to prevent overactivation of the LTR; and (ii) p34Taxmay activate its own promoter both by recruiting critical transcriptionfactors and by releasing transcription repressors. In the absenceof p34Tax, no such transcription factors are available for transcriptionactivation and the LTR cannot be activated even in the absenceof repressors. Therefore deletion or mutation of a repressor sequencedoes not increase the promoter activity of the LTR in the absenceof p34Tax.

cis-acting elements in the U3 region of proviruses are the major determinants for retrovirus tissue tropism at the replicationlevel (8), although sequences outside the LTR may also affectthe tissue tropism of some retroviruses (45). Our results suggestthat BLV transcription varies in different cell types and raisethe possibility that host regulatory factors play an importantrole. This is particularly intriguing, since the tissue tropismof BLV in vivo is now known to extend beyond bovine B lymphocytesto mammary epithelial cells (7) and possibly to T lymphocytes(2, 28) and endothelial cells (34). Tissue-specific and/ordifferentiation-specific proteins may be required for the activationof BLV transcription, as is the case for the human papillomaviruses(39). This is supported by previous observations that BLV expression(virus particles, RNA, or viral proteins) was not detected infreshly isolated peripheral blood lymphocytes of animals infectedwith the virus or in BLV-positive tumor cells, but these cellswere able to produce virus after 24 to 48 h in culture (reviewedin reference 24). Virus production was further increased withmitogens such as concanavalin A, lipopolysaccharide, and pokeweedmitogen (3, 11, 41). In vivo, positive lymphocytes weredetected only in lymph nodes, where B cells would be undergoingdifferentiation to plasma cells (19).

Expression of BLV appears to be regulated by soluble host factors (41, 48, 49). Zandomeni et al. reported that bothstimulatory and inhibitory factors are present in plasma and lymphaticfluid of infected cows. After removal of the stimulatory factor,the inhibitory activity can consistently be detected. Althoughthese investigators identified the host inhibitory factor as amolecule that binds to immunoglobulin G, the nature of the inhibitoryfactor is still unclear and even less is known about the molecularmechanisms involved in this phenomenon. It is possible that NREsin the U3 region of the BLV LTR are the target for this host inhibitoryfactor, which may be responsible for BLV latency. A possible advantageof an NRE is to keep BLV expression at a low level in vivo andhence to reduce the host immune response to the virus.

In this research, we have for the first time delineated in vivo protein-DNA interactions in the entire U3 region of BLV andsystematically analyzed the interaction sites by site-directedmutagenesis. Similar work has not been reported for any memberof the HTLV/BLV group of retroviruses. Based on our data, we proposethat the U3 region of BLV LTR consists of four functional units(Fig. 6): the core promoter region; two positive regulatory elements(the 5' region of the U3 region containing the DR1 and part ofDR3 containing CRE3), and a dually functional region containingthe cis-acting elements CRE2, AP4-2, and the NF- $kappa$ B site. Althoughsite-directed mutagenesis was not performed in the first 60 nucleotidesof the U3 5' region, previous studies by Derse showed that thisregion is an enhancer element. Further experiments testing theexpression pattern of recombinant viruses containing mutationsin these regions in different cell types are necessary to determineif this dually functional region is responsible for the latentstatus of BLV in vivo in infected peripheral B lymphocytes andtumor cells.

	ACKNOWLEDGMENTS

We gratefully acknowledge Caroline Kane and George Sensabaugh for helpful advice, and we thank numerous colleagues (namedin the text) for gifts of cell lines and plasmids.

This study was partially supported by the Vice Chancellor's Research Fund from the University of California, Berkeley; theGrossman Endowment from the School of Public Health, Universityof California, Berkeley; and a grant-in-aid award from Sigma Xi.J.X. was supported by Graduate Fellowships from the Graduate Division,University of California, Berkeley, and by a Levine Fellowshipfrom the School of Public Health, University of California, Berkeley.

	FOOTNOTES

^* Corresponding author. Mailing address: 140 Warren Hall, School of Public Health, University of California, Berkeley, CA 94720.Phone: (510) 642-3870. Fax: (510) 642-6530. E-mail: buehring{at}uclink4.berkeley.edu.

Present address: School of Dentistry, Department of Stomatology, University of California, San Francisco, CA 94143.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Adam, E., P. Kerkhofs, M. Mammerickx, R. Kettmann, A. Burny, L. Droogmans, and L. Willems. 1994. Involvement of the cyclic AMP-responsive element binding protein in bovine leukemia virus expression in vivo. J. Virol. 68:5845-5853[Abstract/Free Full Text].

2. Allen, L. J., M. B. Kabbur, J. S. Cullor, I. A. Gardner, J. L. Stott, and L. W. George. 1996. Alterations in blood lymphocyte subpopulations and hematologic values in neonatal calves after administration of a combination of multiple-antigen vaccines. J. Am. Vet. Med. Assoc. 209:638-642[Medline].

3. Baliga, V., and J. Ferrer. 1977. Expression of the bovine leukemia virus and its internal antigen in blood lymphocytes. Proc. Soc. Exp. Biol. Med. 156:388[Medline].

4. Boros, I. M., F. Tie, and C. Z. Giam. 1995. Interaction of bovine leukemia virus transactivator Tax with bZip proteins. Virology 214:207-214[Medline].

5. Bramblett, D., C. L. Hsu, M. Lozano, K. Earnest, C. Fabritius, and J. Dudley. 1995. A redundant nuclear protein binding site contributes to negative regulation of the mouse mammary tumor virus long terminal repeat. J. Virol. 69:7868-7876[Abstract].

6. Brooks, P. A., J. K. Nyborg, and G. L. Cockrell. 1995. Identification of an NF- $kappa$ B binding site in the bovine leukemia virus promoter. J. Virol. 69:6005-6009[Abstract].

7. Buehring, G. C., P. M. Kramme, and R. D. Schultz. 1994. Evidence for bovine leukemia virus in mammary epithelial cells of infected cows. Lab. Invest. 71:359-365[Medline].

8. Coffin, J. M. 1990. In Retroviridae and their replication, 2nd ed., vol. 1. Raven Press, New York, N.Y.

9. Derse, D. 1987. Bovine leukemia virus transcription is controlled by a virus-encoded trans-acting factor and by cis-acting response elements. J. Virol. 61:2462-2471[Abstract/Free Full Text].

10. Derse, D., and J. W. Casey. 1986. Two elements in the bovine leukemia virus long terminal repeat that regulate gene expression. Science 231:1437-1440[Abstract/Free Full Text].

11. Djilali, S., A. Parodi, and D. Levy. 1987. Bovine leukemia virus replicates in sheep B-lymphocytes under a T-cell released factor. Eur. J. Cancer Clin. Oncol. 23:81[Medline].

12. Epstein, M. A., and Y. M. Barr. 1965. Characterization and mode of growth of a tissue culture strain (EB1) of human lymphoblasts from Burkitt's lymphoma. J. Natl. Cancer Inst. 34:231-240.

13. Fong, A. M., and S. A. Santoro. 1994. Transcriptional regulation of alpha IIb integrin gene expression during megakaryocytic differentiation of K562 cells: role of a silencer element. J. Biol. Chem. 269:18441-18447[Abstract/Free Full Text].

14. Fong, C. L., and D. F. Mark. 1995. The NF-kappa B-like site in the TNF-alpha repressor element is essential for its repressor function. Biochem. Biophys. Res. Commun. 212:879-886[Medline].

15. Goldring, C. E., R. Narayanan, P. Lagadec, and J. F. Jeannin. 1995. Transcriptional inhibition of the inducible nitric oxide synthase gene by competitive binding of NF-kappa B/Rel proteins. Biochem. Biophys. Res. Commun. 209:73-79[Medline].

16. Graves, D. C., and J. F. Ferrer. 1976. In vitro transmission and propagation of the bovine leukemia virus in monolayer cell cultures. Cancer Res. 36:4152-4159[Abstract/Free Full Text].

17. Grayson, J., R. S. Williams, Y. T. Yu, and R. Bassel-Duby. 1995. Synergistic interactions between heterologous upstream activation elements and specific TATA sequences in a muscle-specific promoter. Mol. Cell. Biol. 15:1870-1878[Abstract].

18. Hartig, E., B. Nierlich, S. Mink, G. Nebl, and A. C. Cato. 1993. Regulation of expression of mouse mammary tumor virus through sequences located in the hormone response element: involvement of cell-cell contact and a negative regulatory factor. J. Virol. 67:813-821[Abstract/Free Full Text].

19. Heeney, J. L., P. J. Valli, R. M. Jacobs, and V. E. Valli. 1992. Evidence for bovine leukemia virus infection of peripheral blood monocytes and limited antigen expression in bovine lymphoid tissue. Lab. Invest. 66:608-617[Medline].

20. Hirano, A., and T. Wong. 1988. Functional interaction between transcriptional elements in the long terminal repeat of reticuloendotheliosis virus: cooperative DNA binding of promoter- and enhancer-specific factors. Mol. Cell. Biol. 8:5232-5244[Abstract/Free Full Text].

21. Hoover, T., J. Mikovits, D. Court, Y. L. Liu, H. F. Kung, and Raziuddin. 1996. A nuclear matrix-specific factor that binds a specific segment of the negative regulatory element (NRE) of HIV-1 LTR and inhibits NF-kappa(B) activity. Nucleic Acids Res. 24:1895-1900[Abstract/Free Full Text].

22. Horikoshi, M., T. Hai, Y. S. Lin, M. R. Green, and R. G. Roeder. 1988. Transcription factor ATF interacts with the TATA factor to facilitate establishment of a preinitiation complex. Cell 54:1033-1042[Medline].

23. Katoh, I., Y. Yoshinaka, and Y. Ikawa. 1989. Bovine leukemia virus transactivator p34Tax activates heterologous promoters with a common sequence known as a cAMP-responsive element or the binding site of a cellular transcription factor ATF. EMBO J. 8:497-503[Medline].

24. Kettmann, R., A. Burny, I. Callebaut, L. Droogmans, M. Mammerickx, L. Willems, and D. Portetelle. 1994. In Bovine leukemia virus, 3rd ed., vol. 3. Plenum Press, New York, N.Y.

25. Kiss-Toth, E., S. Paca-uccaralertkun, I. Unk, and I. Boros. 1993. Member of the CREB/ATF protein family, but not CREB alpha plays an active role in BLV tax transactivation in vivo. Nucleic Acids Res. 21:3677-3682[Abstract/Free Full Text].

26. Lasfargues, E. Y., B. Kramarsky, N. H. Sarkar, J. C. Lasfargues, and D. H. Moore. 1972. An established RIII mouse mammary tumor cell line: kinetics of mouse mammary tumor virus (MTV) production. Proc. Soc. Exp. Biol. Med. 139:242-247[Medline].

27. Luckow, B., and G. Schutz. 1987. CAT constructions with multiple unique restriction sites for the functional analysis of eukaryotic promoters and regulatory elements. Nucleic Acids Res. 15:5490[Free Full Text].

28. Murakami, K., K. Okada, H. Amanuma, and Y. Aida. 1994. The gamma delta T cell population in sheep experimentally infected with bovine leukemia virus. Vet. Pathol. 31:103-105[Medline].

29. Niermman, G., and G. C. Buehring. 1997. Hormone regulation of bovine leukemia virus. Virology 239:249-258[Medline].

30. Parekh, B. S., and G. W. Hatfield. 1996. Transcriptional activation by protein-induced DNA bending: evidence for a DNA structural transmission model. Proc. Natl. Acad. Sci. USA 93:1173-1177[Abstract/Free Full Text].

31. Pfeifer, G. P., and A. D. Riggs. 1993. Genomic footprinting by ligation mediated polymerase chain reaction. Methods Mol. Biol. 15:153-168.

32. Pulvertaft, J. V. 1964. Cytology of Burkitt's tumor (African lymphoma). Lancet i:238-240.

33. Rashtchian, A., C. G. Thornton, and G. Heidecker. 1992. A novel method for site-directed mutagenesis using PCR and uracil DNA glycosylase. PCR Methods Appl. 2:124-130[Medline].

34. Rovnak, J., J. W. Casey, A. L. Boyd, M. A. Gonda, and G. L. Cockerell. 1992. Isolation of bovine leukemia virus infected endothelial cells from cattle with persistent lymphocytosis. Lab. Invest. 65:192-202[Medline].

35. Sagata, N., T. Yuanaga, J. Tsuzuku-Kawamura, K. Phishi, and Y. Igawa. 1985. Complete nucleotide sequence of the genome of bovine leukemia virus: its evolutionary relationship to other retroviruses. Proc. Natl. Acad. Sci. USA 82:677-681[Abstract/Free Full Text].

36. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. In Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

37. Sanger, F., S. Nicklen, and A. R. Coulson. 1977. A rapid method for determining sequences in DNA by primed synthesis with DNA polymerase. J. Mol. Biol. 94:441.

38. Soule, H. D., J. Vazquez, A. Long, S. Albert, and M. Brennan. 1973. A human cell line from a pleural effusion derived from breast carcinoma. J. Natl. Cancer Inst. 51:1409-1413.

39. Stoler, M. H., S. M. Wolinsky, A. Whitbeck, T. R. Broker, and L. T. Chow. 1989. Differentiation-linked human papilloma virus types 6 and 11 transcription in genital condylomata revealed by in situ hybridization with message-specific RNA probes. Virology 172:331-340[Medline].

40. Swingler, S., A. Morris, and A. Easton. 1994. Tumour necrosis factor alpha and interleukin-1 beta induce specific subunits of NFKB to bind the HIV-1 enhancer: characterization of transcription factors controlling human immunodeficiency virus type 1 gene expression in neural cells. Biochem. Biophys. Res. Commun. 203:623-630[Medline].

41. Taylor, J. A., and R. M. Jacobs. 1993. Effects of plasma and serum on the in vitro expression of bovine leukemia virus. Lab. Invest. 69:340-346[Medline].

42. Unk, I., E. Kiss-Toth, and I. Boros. 1994. Transcription factor AP-4 participates in activation of bovine leukemia virus long terminal repeat by p34 Tax. Nucleic Acids Res. 22:4872-4875[Abstract/Free Full Text].

43. Van der Maaten, M. J., and J. M. Miller. 1976. Replication of bovine leukemia virus in monolayer cell cultures. Int. J. Cancer 31:791.

44. Willems, L., R. Kettmann, G. Chen, D. Portetelle, A. Burny, and D. Derse. 1992. A cyclic AMP-responsive DNA-binding protein (CREB2) is a cellular transactivator of the bovine leukemia virus long terminal repeat. J. Virol. 66:766-772[Abstract/Free Full Text].

45. Wolff, L., and S. Ruscetti. 1986. Tissue tropism of a leukemogenic murine retrovirus is determined by sequences outside of the long terminal repeats. Proc. Natl. Acad. Sci. USA 83:3376-3380[Abstract/Free Full Text].

45a. Xiao, J., and G. C. Buehring. Submitted for publication.

46. Xu, X., D. A. Brown, I. Kitajima, J. Bilakovics, L. W. Fey, and M. I. Nerenberg. 1994. Transcriptional suppression of the human T-cell leukemia virus type I long terminal repeat occurs by an unconventional interaction of a CREB factor with the R region. Mol. Cell. Biol. 14:5371-5383[Abstract/Free Full Text].

47. Yeh, C. H., and A. J. Shatkin. 1994. Down-regulation of Rous sarcoma virus long terminal repeat promoter activity by a HeLa cell basic protein. Proc. Natl. Acad. Sci. USA 91:11002-11006[Abstract/Free Full Text].

48. Zandomeni, R. O., M. Carrera-Zandomeni, E. Esteban, W. Donawick, and J. F. Ferrer. 1992. Induction and inhibition of bovine leukaemia virus expression in naturally infected cells. J. Gen. Virol. 73:1915-1924[Abstract/Free Full Text].

49. Zandomeni, R. O., E. Esteban, M. Carrera-Zandomeni, and J. F. Ferrer. 1994. Host soluble factors with blocking and stimulating activity on the expression of the bovine leukemia virus. J. Infect. Dis. 170:787-794[Medline].

This article has been cited by other articles:

Calomme, C., Dekoninck, A., Nizet, S., Adam, E., Nguyen, T. L.-A., Van Den Broeke, A., Willems, L., Kettmann, R., Burny, A., Van Lint, C. (2004). Overlapping CRE and E Box Motifs in the Enhancer Sequences of the Bovine Leukemia Virus 5' Long Terminal Repeat Are Critical for Basal and Acetylation-Dependent Transcriptional Activity of the Viral Promoter: Implications for Viral Latency. J. Virol. 78: 13848-13864 [Abstract] [Full Text]
Nguyen, T. L.-A., Calomme, C., Wijmeersch, G., Nizet, S., Veithen, E., Portetelle, D., de Launoit, Y., Burny, A., Van Lint, C. (2004). Deacetylase Inhibitors and the Viral Transactivator TaxBLV Synergistically Activate Bovine Leukemia Virus Gene Expression via a cAMP-responsive Element- and cAMP-responsive Element-binding Protein-dependent Mechanism. J. Biol. Chem. 279: 35025-35036 [Abstract] [Full Text]
Xiao, J., Jethanandani, P., Ziober, B. L., Kramer, R. H. (2003). Regulation of {alpha}7 Integrin Expression during Muscle Differentiation. J. Biol. Chem. 278: 49780-49788 [Abstract] [Full Text]
Merezak, C., Reichert, M., Van Lint, C., Kerkhofs, P., Portetelle, D., Willems, L., Kettmann, R. (2002). Inhibition of Histone Deacetylases Induces Bovine Leukemia Virus Expression In Vitro and In Vivo. J. Virol. 76: 5034-5042 [Abstract] [Full Text]
Calomme, C., Nguyen, T. L.-A., de Launoit, Y., Kiermer, V., Droogmans, L., Burny, A., Van Lint, C. (2002). Upstream Stimulatory Factors Binding to an E Box Motif in the R Region of the Bovine Leukemia Virus Long Terminal Repeat Stimulates Viral Gene Expression. J. Biol. Chem. 277: 8775-8789 [Abstract] [Full Text]
Merezak, C., Pierreux, C., Adam, E., Lemaigre, F., Rousseau, G. G., Calomme, C., Van Lint, C., Christophe, D., Kerkhofs, P., Burny, A., Kettmann, R., Willems, L. (2001). Suboptimal Enhancer Sequences Are Required for Efficient Bovine Leukemia Virus Propagation In Vivo: Implications for Viral Latency. J. Virol. 75: 6977-6988 [Abstract] [Full Text]
Tajima, S., Aida, Y. (2000). The Region between Amino Acids 245 and 265 of the Bovine Leukemia Virus (BLV) Tax Protein Restricts Transactivation Not Only via the BLV Enhancer but Also via Other Retrovirus Enhancers. J. Virol. 74: 10939-10949 [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 Xiao, J.
	Articles by Buehring, G. C.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Xiao, J.
	Articles by Buehring, G. C.

1.	Adam, E., P. Kerkhofs, M. Mammerickx, R. Kettmann, A. Burny, L. Droogmans, and L. Willems. 1994. Involvement of the cyclic AMP-responsive element binding protein in bovine leukemia virus expression in vivo. J. Virol. 68:5845-5853[Abstract/Free Full Text].
2.	Allen, L. J., M. B. Kabbur, J. S. Cullor, I. A. Gardner, J. L. Stott, and L. W. George. 1996. Alterations in blood lymphocyte subpopulations and hematologic values in neonatal calves after administration of a combination of multiple-antigen vaccines. J. Am. Vet. Med. Assoc. 209:638-642[Medline].
3.	Baliga, V., and J. Ferrer. 1977. Expression of the bovine leukemia virus and its internal antigen in blood lymphocytes. Proc. Soc. Exp. Biol. Med. 156:388[Medline].
4.	Boros, I. M., F. Tie, and C. Z. Giam. 1995. Interaction of bovine leukemia virus transactivator Tax with bZip proteins. Virology 214:207-214[Medline].
5.	Bramblett, D., C. L. Hsu, M. Lozano, K. Earnest, C. Fabritius, and J. Dudley. 1995. A redundant nuclear protein binding site contributes to negative regulation of the mouse mammary tumor virus long terminal repeat. J. Virol. 69:7868-7876[Abstract].
6.	Brooks, P. A., J. K. Nyborg, and G. L. Cockrell. 1995. Identification of an NF- $kappa$ B binding site in the bovine leukemia virus promoter. J. Virol. 69:6005-6009[Abstract].
7.	Buehring, G. C., P. M. Kramme, and R. D. Schultz. 1994. Evidence for bovine leukemia virus in mammary epithelial cells of infected cows. Lab. Invest. 71:359-365[Medline].
8.	Coffin, J. M. 1990. In Retroviridae and their replication, 2nd ed., vol. 1. Raven Press, New York, N.Y.
9.	Derse, D. 1987. Bovine leukemia virus transcription is controlled by a virus-encoded trans-acting factor and by cis-acting response elements. J. Virol. 61:2462-2471[Abstract/Free Full Text].
10.	Derse, D., and J. W. Casey. 1986. Two elements in the bovine leukemia virus long terminal repeat that regulate gene expression. Science 231:1437-1440[Abstract/Free Full Text].
11.	Djilali, S., A. Parodi, and D. Levy. 1987. Bovine leukemia virus replicates in sheep B-lymphocytes under a T-cell released factor. Eur. J. Cancer Clin. Oncol. 23:81[Medline].
12.	Epstein, M. A., and Y. M. Barr. 1965. Characterization and mode of growth of a tissue culture strain (EB1) of human lymphoblasts from Burkitt's lymphoma. J. Natl. Cancer Inst. 34:231-240.
13.	Fong, A. M., and S. A. Santoro. 1994. Transcriptional regulation of alpha IIb integrin gene expression during megakaryocytic differentiation of K562 cells: role of a silencer element. J. Biol. Chem. 269:18441-18447[Abstract/Free Full Text].
14.	Fong, C. L., and D. F. Mark. 1995. The NF-kappa B-like site in the TNF-alpha repressor element is essential for its repressor function. Biochem. Biophys. Res. Commun. 212:879-886[Medline].
15.	Goldring, C. E., R. Narayanan, P. Lagadec, and J. F. Jeannin. 1995. Transcriptional inhibition of the inducible nitric oxide synthase gene by competitive binding of NF-kappa B/Rel proteins. Biochem. Biophys. Res. Commun. 209:73-79[Medline].
16.	Graves, D. C., and J. F. Ferrer. 1976. In vitro transmission and propagation of the bovine leukemia virus in monolayer cell cultures. Cancer Res. 36:4152-4159[Abstract/Free Full Text].
17.	Grayson, J., R. S. Williams, Y. T. Yu, and R. Bassel-Duby. 1995. Synergistic interactions between heterologous upstream activation elements and specific TATA sequences in a muscle-specific promoter. Mol. Cell. Biol. 15:1870-1878[Abstract].
18.	Hartig, E., B. Nierlich, S. Mink, G. Nebl, and A. C. Cato. 1993. Regulation of expression of mouse mammary tumor virus through sequences located in the hormone response element: involvement of cell-cell contact and a negative regulatory factor. J. Virol. 67:813-821[Abstract/Free Full Text].
19.	Heeney, J. L., P. J. Valli, R. M. Jacobs, and V. E. Valli. 1992. Evidence for bovine leukemia virus infection of peripheral blood monocytes and limited antigen expression in bovine lymphoid tissue. Lab. Invest. 66:608-617[Medline].
20.	Hirano, A., and T. Wong. 1988. Functional interaction between transcriptional elements in the long terminal repeat of reticuloendotheliosis virus: cooperative DNA binding of promoter- and enhancer-specific factors. Mol. Cell. Biol. 8:5232-5244[Abstract/Free Full Text].
21.	Hoover, T., J. Mikovits, D. Court, Y. L. Liu, H. F. Kung, and Raziuddin. 1996. A nuclear matrix-specific factor that binds a specific segment of the negative regulatory element (NRE) of HIV-1 LTR and inhibits NF-kappa(B) activity. Nucleic Acids Res. 24:1895-1900[Abstract/Free Full Text].
22.	Horikoshi, M., T. Hai, Y. S. Lin, M. R. Green, and R. G. Roeder. 1988. Transcription factor ATF interacts with the TATA factor to facilitate establishment of a preinitiation complex. Cell 54:1033-1042[Medline].
23.	Katoh, I., Y. Yoshinaka, and Y. Ikawa. 1989. Bovine leukemia virus transactivator p34Tax activates heterologous promoters with a common sequence known as a cAMP-responsive element or the binding site of a cellular transcription factor ATF. EMBO J. 8:497-503[Medline].
24.	Kettmann, R., A. Burny, I. Callebaut, L. Droogmans, M. Mammerickx, L. Willems, and D. Portetelle. 1994. In Bovine leukemia virus, 3rd ed., vol. 3. Plenum Press, New York, N.Y.
25.	Kiss-Toth, E., S. Paca-uccaralertkun, I. Unk, and I. Boros. 1993. Member of the CREB/ATF protein family, but not CREB alpha plays an active role in BLV tax transactivation in vivo. Nucleic Acids Res. 21:3677-3682[Abstract/Free Full Text].
26.	Lasfargues, E. Y., B. Kramarsky, N. H. Sarkar, J. C. Lasfargues, and D. H. Moore. 1972. An established RIII mouse mammary tumor cell line: kinetics of mouse mammary tumor virus (MTV) production. Proc. Soc. Exp. Biol. Med. 139:242-247[Medline].
27.	Luckow, B., and G. Schutz. 1987. CAT constructions with multiple unique restriction sites for the functional analysis of eukaryotic promoters and regulatory elements. Nucleic Acids Res. 15:5490[Free Full Text].
28.	Murakami, K., K. Okada, H. Amanuma, and Y. Aida. 1994. The gamma delta T cell population in sheep experimentally infected with bovine leukemia virus. Vet. Pathol. 31:103-105[Medline].
29.	Niermman, G., and G. C. Buehring. 1997. Hormone regulation of bovine leukemia virus. Virology 239:249-258[Medline].
30.	Parekh, B. S., and G. W. Hatfield. 1996. Transcriptional activation by protein-induced DNA bending: evidence for a DNA structural transmission model. Proc. Natl. Acad. Sci. USA 93:1173-1177[Abstract/Free Full Text].
31.	Pfeifer, G. P., and A. D. Riggs. 1993. Genomic footprinting by ligation mediated polymerase chain reaction. Methods Mol. Biol. 15:153-168.
32.	Pulvertaft, J. V. 1964. Cytology of Burkitt's tumor (African lymphoma). Lancet i:238-240.
33.	Rashtchian, A., C. G. Thornton, and G. Heidecker. 1992. A novel method for site-directed mutagenesis using PCR and uracil DNA glycosylase. PCR Methods Appl. 2:124-130[Medline].
34.	Rovnak, J., J. W. Casey, A. L. Boyd, M. A. Gonda, and G. L. Cockerell. 1992. Isolation of bovine leukemia virus infected endothelial cells from cattle with persistent lymphocytosis. Lab. Invest. 65:192-202[Medline].
35.	Sagata, N., T. Yuanaga, J. Tsuzuku-Kawamura, K. Phishi, and Y. Igawa. 1985. Complete nucleotide sequence of the genome of bovine leukemia virus: its evolutionary relationship to other retroviruses. Proc. Natl. Acad. Sci. USA 82:677-681[Abstract/Free Full Text].
36.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. In Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
37.	Sanger, F., S. Nicklen, and A. R. Coulson. 1977. A rapid method for determining sequences in DNA by primed synthesis with DNA polymerase. J. Mol. Biol. 94:441.
38.	Soule, H. D., J. Vazquez, A. Long, S. Albert, and M. Brennan. 1973. A human cell line from a pleural effusion derived from breast carcinoma. J. Natl. Cancer Inst. 51:1409-1413.
39.	Stoler, M. H., S. M. Wolinsky, A. Whitbeck, T. R. Broker, and L. T. Chow. 1989. Differentiation-linked human papilloma virus types 6 and 11 transcription in genital condylomata revealed by in situ hybridization with message-specific RNA probes. Virology 172:331-340[Medline].
40.	Swingler, S., A. Morris, and A. Easton. 1994. Tumour necrosis factor alpha and interleukin-1 beta induce specific subunits of NFKB to bind the HIV-1 enhancer: characterization of transcription factors controlling human immunodeficiency virus type 1 gene expression in neural cells. Biochem. Biophys. Res. Commun. 203:623-630[Medline].
41.	Taylor, J. A., and R. M. Jacobs. 1993. Effects of plasma and serum on the in vitro expression of bovine leukemia virus. Lab. Invest. 69:340-346[Medline].
42.	Unk, I., E. Kiss-Toth, and I. Boros. 1994. Transcription factor AP-4 participates in activation of bovine leukemia virus long terminal repeat by p34 Tax. Nucleic Acids Res. 22:4872-4875[Abstract/Free Full Text].
43.	Van der Maaten, M. J., and J. M. Miller. 1976. Replication of bovine leukemia virus in monolayer cell cultures. Int. J. Cancer 31:791.
44.	Willems, L., R. Kettmann, G. Chen, D. Portetelle, A. Burny, and D. Derse. 1992. A cyclic AMP-responsive DNA-binding protein (CREB2) is a cellular transactivator of the bovine leukemia virus long terminal repeat. J. Virol. 66:766-772[Abstract/Free Full Text].
45.	Wolff, L., and S. Ruscetti. 1986. Tissue tropism of a leukemogenic murine retrovirus is determined by sequences outside of the long terminal repeats. Proc. Natl. Acad. Sci. USA 83:3376-3380[Abstract/Free Full Text].
45a.	Xiao, J., and G. C. Buehring. Submitted for publication.
46.	Xu, X., D. A. Brown, I. Kitajima, J. Bilakovics, L. W. Fey, and M. I. Nerenberg. 1994. Transcriptional suppression of the human T-cell leukemia virus type I long terminal repeat occurs by an unconventional interaction of a CREB factor with the R region. Mol. Cell. Biol. 14:5371-5383[Abstract/Free Full Text].
47.	Yeh, C. H., and A. J. Shatkin. 1994. Down-regulation of Rous sarcoma virus long terminal repeat promoter activity by a HeLa cell basic protein. Proc. Natl. Acad. Sci. USA 91:11002-11006[Abstract/Free Full Text].
48.	Zandomeni, R. O., M. Carrera-Zandomeni, E. Esteban, W. Donawick, and J. F. Ferrer. 1992. Induction and inhibition of bovine leukaemia virus expression in naturally infected cells. J. Gen. Virol. 73:1915-1924[Abstract/Free Full Text].
49.	Zandomeni, R. O., E. Esteban, M. Carrera-Zandomeni, and J. F. Ferrer. 1994. Host soluble factors with blocking and stimulating activity on the expression of the bovine leukemia virus. J. Infect. Dis. 170:787-794[Medline].