E1A promoter of bovine adenovirus type 3

doi:10.1099/vir.0.82108-0

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E1A promoter of bovine adenovirus type 3

Li Xing and Suresh Kumar Tikoo

Vectored Vaccine Program, Vaccine and Infectious Disease Organization, 120 Veterinary Road, University of Saskatchewan, Saskatoon, SK S7N 5E3, Canada

Correspondence
Suresh Kumar Tikoo
Suresh.tik{at}Usask.ca

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Conserved motifs of eukaryotic gene promoters, such as TATAbox and CAAT box sequences, of E1A of human adenoviruses (e.ghuman adenovirus 5) lie between the left inverted terminal repeat(ITR) and the ATG of E1A. However, analysis of the left endof the bovine adenovirus 3 (BAdV-3) genome revealed that theconserved sequences of the E1A promoter are present only inthe ITR. As such, the promoter activity of ITR was tested inthe context of a BAdV-3 vector or a plasmid-based system. Differentregions of the left end of the BAdV-3 genome initiated transcriptionof the red fluorescent protein gene in a plasmid-based system.Moreover, BAdV-3 mutants in which the open reading frame ofE1A was placed immediately downstream of the ITR produced E1Atranscript and could be propagated in non-E1A-complementingMadin–Darby bovine kidney cells. These results suggestthat the left ITR contains the sole BAdV-3 E1A promoter.

${dagger}$ Present address: Channing Laboratory, Brigham and Women's Hospital,Department of Medicine and Department of Microbiology and MolecularGenetics, Harvard Medical School, 181 Longwood Avenue, Boston,MA 02115, USA.

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Bovine adenovirus 3 (BAdV-3) is being characterized at the molecularlevel to develop gene-transfer vector(s) for gene delivery toanimals (Reddy et al., 1999c; Zakhartchouk et al., 1998, 1999)and humans (Rasmussen et al., 1999). Recently, the nucleotidesequence and the transcription map of the BAdV-3 genome havebeen determined (Baxi et al., 1999; Idamakanti et al., 1999;Reddy et al., 1998c, 1999a; Zheng et al., 1999). The E1 regionof BAdV-3, located at the left end of the viral genome, consistsof the E1A and E1B transcription units (Reddy et al., 1999a;van Olphen et al., 2002). The E1A transcriptional unit, locatedbetween 0.8 and 10.5 map units (m.u.), produces several differenttranscripts that encode phosphoproteins of 43, 57 and 65 kDa.The E1B transcriptional unit, located between 4.2 and 10.5 m.u.,overlaps that of E1A and encodes phosphoproteins of 19 and 48 kDa.In this report, by using E1A 5'-flanking region mutants, weevaluated the promoter activity of the left inverted terminalrepeat (ITR) of BAdV-3.

The ITRs of human, canine, porcine and simian adenoviruses (membersof the genus Mastadenovirus) contain conserved sequence motifsthat bind cellular transcriptional factors SpI and ATF (Dánet al., 2001), which are responsible for the promoter activityof the ITR (Hatfield & Hearing, 1991). However, E1A of theseadenoviruses also contains promoter-like elements located betweenthe left ITR and the ATG of E1A (Davison et al., 2003).

Unlike in other members of the genus Mastadenovirus, includinghuman adenovirus 5 (HAdV-5; Hearing & Shenk, 1983, 1986),porcine adenovirus 3 (PAdV-3; Xing & Tikoo, 2004, 2005),mouse adenovirus 1 (Meissner et al., 1997) and canine adenovirus1 (Morrison et al., 1997), we could not find conserved motifsof eukaryotic gene promoters, such as TATA box and CAAT boxsequences, between the left ITR and the ATG of E1A of BAdV-3.The software program I (Reese et al., 1996) suggests that theE1A gene is under the control of a TATA-less promoter that islocated mainly in the ITR (between nt 94 and 211). The regionbetween nt 94 and 211 contains GC-rich sequences, which arebelieved to be SP1-binding sites (Hatfield & Hearing, 1993;Kadonaga et al., 1987). However, deletion of 72 bp betweennt 89 and 162, overlapping most of the potential promoter sequencepredicted by program I, did not seem to have any effect on thekinetics of virus replication compared with those of wild-typeBAdV-3 (van Olphen & Mittal, 2002), suggesting that GC-richsequences between nt 94 and 211 (Fig. 1a) could not bethe major promoter region of E1A. Program II (Hctata; Milanesi& Rogozin, 1998; Milanesi et al., 1995, 1996, 1999) alsosuggests that the E1A gene promoter is located in the ITR, butit may contain a TATA box (Hampsey, 1998) with the sequence‘TATGA’ between nt 68 and 72. Additionally, theCAAT element of eukaryotic promoters was found between nt 46and 49 (Fig. 1a). Interestingly, although there are conservedmotifs of eukaryotic-like promoters between the left ITR andthe ATG of E1A of BAdV-1 and BAdV-2 (Fig. 1a), there areno such sequence motifs present in the ITR of BAdV-1 and BAdV-2(genus Mastadenovirus). In contrast, conserved motifs of eukaryotic-likepromoters are present in the ITR of BAdV-4 (genus Atadenovirus),which does not possess a recognizable homologue of E1A (Davisonet al., 2003).

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Fig. 1. Analysis of the BAdV-3 promoter. (a) Left ITR (filled box) and 5'-flanking sequences of BAdV E1A ORF (thin line). Numbers designate the nucleotide positions relative to the left terminus of the respective BAdV genomes [BAdV-1 (GenBank accession no. NC_006324); BAdV-2 (AF252854); BAdV-3 (AF030154); BAdV-4 (AF036092)]. (b) Left ITR (filled box), 5'-flanking sequences of BAdV-3 E1A ORF (thin line) and cis-acting packaging domain (open box). Numbers designate the nucleotide positions relative to the left terminus of the BAdV-3 genome. (c) PAdV-3 or BAdV-3 genome sequences (open arrows). Numbers designate the nucleotide positions relative to the left terminus of the corresponding virus genome. Arrows also indicate the direction of mRNA transcription. (d) Products of RT-PCR using DNase-treated RNA isolated from cells transfected with indicated plasmid DNA were synthesized by using a primer pair specific for RFP as described in the text. RNA with reverse transcriptase (+); RNA without reverse transcriptase (–). MassRuler DNA ladder mix DNA (Fermentas) was used as size marker (M). The expected band size is shown on the right. (e) The cells were transfected with 2 µg pDsRed2-N1 (P), pDsRed2-NP (N), pDsRedpav1 (1), pDsRedpav2 (2), pDsRedbav1 (3) or pDsRedbav2 (4) plasmid DNA. After 48 h, transfected cells were analysed by fluorescence microscopy. (i) Fluorescence; (ii) phase contrast.

The promoter activity in the ITR of adenoviruses is well established(Hatfield & Hearing, 1991

; Ooyama et al., 1989

; Xing &Tikoo, 2005

; Yamamoto et al., 2003

). To test the in vitro promoteractivity of BAdV-3 E1A transcriptional-control sequences (Fig. 1b

),we constructed plasmids in which the red fluorescence protein(RFP)-encoding gene was placed under the control of BAdV-3 DNAsequences (Reddy et al., 1998c

), between nt 1 and 224 (pDsRedbav1)or between nt 1 and 601 (pDsRedbav2) (Fig. 1c

). PlasmidpDsRed2-N1 contains the RFP gene under the control of the humancytomegalovirus immediate-early promoter and plasmid pDsRed2-NPcontains the RFP gene without any transcriptional-control elementat the 5' end. For comparison purposes, we also constructedplasmids in which the RFP gene was under the control of PAdV-3DNA sequences (Reddy et al., 1998a

, b

) between nt 1 and 151(pDsRedpav1) or nt 1 and 495 (pDsRedpav2) (Fig. 1c

). Initially,the promoter activity was analysed by RT-PCR using specificprimers. Different cells were transfected with individual plasmids.At 72 h post-transfection, the cells were collected andtotal RNA was isolated and analysed as described previously(Zakhartchouk et al., 2004

), using RFP gene-specific primers(RFPF, 5'-ATGGCCTCCTCCGAGAACGTCAT-3'; RFPR, 5'-CTACAGGAACAGGTGGTGGC-3').As seen in Fig. 1(d)

, an RFP gene-specific RT-PCR productof the expected size could be detected in cells transfectedwith plasmid pDsRedpav2 (lane +) or plasmid pDsRedbav2 (lane+). The RNA sample controls with no reverse transcriptase didnot show any bands (lane –), indicating that the 680 bpfragment was amplified from RFP mRNA and not from the residualDNA. Moreover, no such product could be detected in cells transfectedwith pDsRedpav1 or pDsRedbav1 (data not shown). To confirm expressionof the RFP protein, the transfected cells were analysed by fluorescencemicroscopy. Representative results are shown in Fig. 1(e)

.Expression of RFP could be detected in human 293 (Graham etal., 1977

), bovine VIDO R2 (Reddy et al., 1999c

) and porcineVIDO R1 (Reddy et al., 1999b

) cells transfected with plasmidpDsRedpav2 (column 2), but not with plasmid pDsRedpav1 (column1). Similarly, expression of RFP could be detected in cellstransfected with plasmid pDsRedbav2 (column 4), but not withpDsRedbav1 (column 3). These results suggest that, as in PAdV-3(Xing & Tikoo, 2005

), the 5'-flanking sequences of the BAdV-3E1A display promoter activity in vitro. Transcription from someregions of the left end of the HAdV-5 genome has not been detectedin a plasmid-based system (Hatfield & Hearing, 1991

As the conserved sequences of eukaryotic promoters are locatedin the ITR (Fig. 1a, b), we investigated the promoter activityof the BAdV-3 left ITR by constructing and analysing a seriesof BAdV-3 mutants (Fig. 2a), designated Bav16 (Bav3-224/468),Bav18 (Bav3-224/541), Bav110 (Bav3-224/552) and Bav112 (Bav3-224/560)(Xing et al., 2003).

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Fig. 2. In vivo promoter activity of the BAdV-3 ITR. (a) The ITR is represented by an open box. The E1A translation start site (ATG) is indicated by an arrowhead. Names of the individual BAdV-3 mutants are given on the left. Deleted sequences are indicated by bold lines. Nucleotide numbers relative to the left terminus of the genome denote the last base pair present on either side of the deletion. (b) MDBK cells were infected with wild-type or mutant BAdV-3 at an m.o.i. of 15 p.f.u. RNA isolated at 36 h post-infection was analysed by Northern hybridization. As a control, rRNAs (18S and 28S) were detected by staining RNA with ethidium bromide in denaturing formaldehyde/agarose gel. (c) The transcription-initiation site(s) of E1A was determined by 5'-RACE experiments as described in the text. Sizes of DNA markers (in bp) are shown on the left. (i) Reverse primer, nt 1327–1344; (ii) reverse primer, nt 1882–1899.

To analyse the transcription of E1A, Madin–Darby bovinekidney (MDBK) cells were infected with wild-type or mutant BAdV-3at an m.o.i. of 40 p.f.u. in the presence of AraC (125 µg ml^–1).Total RNA isolated at 7 h post-infection was separatedin 1 % formaldehyde/agarose gel and analysed by Northern blottingusing a ³²P-labelled E1A-specific DNA probe (nt 560–1156).Although E1A mRNA could be detected in wild-type BAdV-3-infectedcells, the E1A mRNA produced in mutant virus-infected cellswas undetectable (data not shown). This could be due to thesensitivity limitation of Northern blot analysis. Therefore,MDBK cells were infected with mutant BAdV-3 at an m.o.i. of15 p.f.u. in the absence of AraC. Total RNA isolated at36 h post-infection was analysed by Northern hybridizationusing a ³²P-labelled E1A-specific DNA probe (nt 560–1156).As expected, E1A-specific mRNA could be detected in wild-typeBAdV-3-infected cells (Fig. 2b

). Similarly, E1A-specificmRNA could be detected in cells infected with mutants Bav16,Bav18, Bav110 or Bav112. However, the level of E1A mRNA in infectedcells differed between mutant viruses. Mutant Bav16, carryingdeletion of sequences between nt 224 and 468, displayed nearlythe same level of E1A mRNA as wild-type BAdV-3. Cells infectedby mutant Bav18 (nt 224–541), Bav110 (nt 224–552)or Bav112 (nt 224–560) displayed a correspondingly gradualreduction in the accumulation of E1A mRNA compared with wild-typeBAdV-3- or Bav16-infected cells. This could be due to deletionof sequences between nt 224 and 382, which reduces the steady-statelevel of E1A/E1B mRNAs significantly and also affects the mRNAlevels of E2A, E3 and E4 in virus-infected MDBK cells (unpublisheddata). These results suggested that the left ITR directs thetranscription of BAdV-3 E1A, which is regulated by downstreamsequences between the left ITR and the ATG of E1A. Previously,different regions of the left end of the HAdV-5 genome havebeen shown to induce different levels of transcription of areporter gene in vivo (Yamamoto et al., 2003

To determine the E1A transcription start site in these mutants,MDBK cells were infected with mutant BAdVs at an m.o.i. of 15 p.f.u.At 36 h post-infection, total RNA was isolated and amplificationof cDNA 5' ends was performed with a 5'-RACE (rapid amplificationof cDNA ends) kit (Invitrogen) as described previously (Xing& Tikoo, 2005). cDNAs were synthesized by using BAdV-3 E1Agene-specific primers (reverse, nt 1327–1344; reverse,nt 1882–1899). Polydeoxynucleotide-tailed cDNAs were amplifiedby using a nested gene-specific reverse primer (nt 852–869)and a 5'-RACE AAP primer. DNA sequence analysis of PCR products(Fig. 2c) indicated that transcription of the E1A genewas initiated at both nt 286 and nt 560 in wild-type BAdV-3.However, mutants Bav18 (nt 224–541) and Bav112 (nt 224–560)use only one transcription-initiation site at nt 560. In mutantBav16 (nt 224–468), transcription of the E1A gene wasinitiated at nt 500–501, as well as at nt 560. In Bav110(nt 224–552), E1A transcription starts at nt 554 (Zhenget al., 1999). Interestingly, transcription activity of differentregions of the left end of HAdV-5 varied in different organs(Yamamoto et al., 2003).

E1A gene products are required for transactivation of otheradenoviral early genes and, consequently, control adenovirusreplication (Russell, 2000). To determine whether the levelof E1A gene expression directed by the ITR in the absence ofother potential transcriptional-control sequences (between nt224 and 560) is enough to support virus replication in a non-E1A-complementingcell line, MDBK cells were infected with wild-type or mutantBAdV-3 at an m.o.i. of 5 p.f.u. At different times post-infection,infected cells were harvested and amounts of infectious virusprogeny were determined by plaque assay in VIDO R2 cells. Wild-typeBAdV-3 reached a titre of approximately 5x10⁵ p.f.u. ml^–1at 48 h post-infection (Fig. 3a). BAdV-3 mutants displayeda lag in viral growth to varying degrees. Moreover, Bav16, Bav18,Bav110 and Bav112 grew to 0.9, 1.5, 1.7 and 2.0 logs lower thanthe wild-type BAdV-3, respectively (Fig. 3a). These resultssuggested that E1A expression regulated by ITR and its downstreamsequences (between nt 224 and 560) supports the replicationof mutant BAdV-3 in MDBK cells. An earlier report suggestedthat the same region of the HAdV-5 ITR initiated reporter-genetranscription differently in cancer cells and in normal organsin vivo (Yamamoto et al., 2003).

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Fig. 3. Replication of BAdV-3 mutants. (a) Cells were infected with wild-type or mutant BAdV-3 at an m.o.i. of 5 p.f.u. and harvested at indicated times post-infection. Titres were determined by plaque assay in VIDO R2 cells and represent the mean values of three replicates. The results depict the mean of two such experiments. (b) Cells were infected with wild-type or mutant BAdV-3 at an m.o.i. of 5 p.f.u. DNA was prepared at indicated times post-infection. After digestion with EcoRI, the agarose gel-fractionated DNAs were subjected to Southern blot analysis. (c) Results of PhosphorImager scanning of DNA band intensity are shown.

To study further the replication of BAdV-3 mutants, we examinedviral DNA accumulation in mutant virus-infected cells. MDBKcells were infected with mutant viruses at an m.o.i. of 5 p.f.u.per cell. Total DNA isolated at 9, 17 and 33 h post-infectionwas digested with EcoRI and analysed by Southern blot analysisusing a ³²P-labelled DNA probe (nt 828–1651). As expected,all BAdV-3 mutants could replicate in MDBK cells, albeit withvarying efficiency (Fig. 3b, c

). The level of BAdV-3 DNAaccumulation (Fig. 3b, c

) appears to be correlated directlyto the level of E1A mRNA (Fig. 2b

) in MDBK cells.

Although the ITRs of HAdV-5 and PAdV-3 display promoter-likeactivity, the core elements of the E1A promoter are locatedbetween the left ITR and the ATG of E1A (Xing & Tikoo, 2005;Yamamoto et al., 2003). Our results suggest that the core elementsof the BAdV-3 E1A promoter are located in the left ITR. Severallines of evidence support the fact that the left ITR of BAdV-3contains the core promoter element of E1A. First, DNA sequenceanalysis of the left ITR showed the presence of a CCAAT box(nt 45–49), a TATA-like box (nt 68–72) and mostof a GC box (nt 108–209). Second, in the absence of sequencesbetween nt 224 and 560 (Bav112), the promoter activity of theITR is sufficient to express E1A, which supports the replicationof Bav112 and the production of progeny virions in non-E1A-complementingMDBK cells. Third, transcriptional analysis of the E1 regionidentified E1A transcriptional start sites near the left ITR(Reddy et al., 1998c, 1999a; Zheng et al., 1999). Further understandingof the different mechanisms of transcriptional-control regionsof E1A should help to develop improved adenovirus vectors forgene delivery.

ACKNOWLEDGEMENTS

We thank Betty Chow for her technical help. The work was supportedby a grant from the Natural Sciences and Engineering ResearchCouncil (NSERC) of Canada to S. K. T. Published as VIDO articleno. 351.

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Received 6 April 2006; accepted 7 August 2006.

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