Members of the GATA Family of Transcription Factors Bind to the U3 Region of Cas-Br-E and Graffi Retroviruses and Transactivate Their Expression

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J Virol, July 1998, p. 5579-5588, Vol. 72, No. 7
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Members of the GATA Family of Transcription Factors Bind to the U3 Region of Cas-Br-E and Graffi Retroviruses and Transactivate Their Expression

Corinne Barat and Eric Rassart^*

Laboratoire de Biologie Moléculaire, Département de Sciences Biologiques, Université du Québec à Montréal, Montréal, Québec, Canada H3C 3P8

Received 17 October 1997/Accepted 25 March 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Cas-Br-E and Graffi are two murine viruses that induce myeloid leukemia in mice: while Cas-Br-E induces mostly non-T, non-Bleukemia composed of very immature cells, Graffi causes exclusivelya granulocytic leukemia (E. Rassart, J. Houde, C. Denicourt, M.Ru, C. Barat, E. Edouard, L. Poliquin, and D. Bergeron, Curr.Top. Microbiol. Immunol. 211:201-210, 1995). In an attempt tounderstand the basis of the myeloid specificity of these two retroviruses,we used DNase I footprinting analysis and gel mobility shift assaysto identify a number of protein binding sites within the Cas-Br-Eand Graffi U3 regions. Two protected regions include potentialGATA binding sites. Methylation interference analysis with differenthematopoietic nuclear extracts showed the importance of the Gresidues in these GATA sites, and supershift assays clearly identifiedthe binding factors as GATA-1, GATA-2, and GATA-3. Transient assayswith long terminal repeat (LTR)-chloramphenicol acetyltransferaseconstructs showed that these three GATA family members are indeedable to transactivate Cas-Br-E and Graffi LTRs. Thus, the availabilityand relative abundance of the various members of the GATA familyof transcription factors in a given cell type could influencethe transcriptional tissue specificity of murine leukemia virusesand hence their disease specificity.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Nondefective murine leukemia viruses (MuLV) can induce a large spectrum of pathologic responses in mice, with a predominanceof hematopoietic tumors. They do not carry an oncogene, and tumorigenictransformation is usually achieved by retroviral integration atthe vicinity of a cellular proto-oncogene. Although MuLVs caninfect many tissues and cell types, each virus will induce a specifictype of tumor: T or B lymphomas, erythroleukemia, myeloid leukemia,etc. Many studies have shown that the primary determinant forthis disease specificity and for tumorigenicity itself is theviral long terminal repeat (LTR) (11, 19-21, 25, 34, 35,42, 58, 76). Moreover, a very good correlation has beendemonstrated between transcriptional tissue specificity and diseasespecificity: viral gene expression is higher in the cell typethat is the target for oncogenic transformation (6, 12, 32,64).

The U3 region of the LTR contains the promoter and the transcriptional regulatory elements. Since retroviruses use the cellularmachinery for gene expression (transcription, translation), theyare also likely to use the cellular regulatory functions, includingtranscription factors. Indeed, dissection of retroviral promoter-enhancerregions has led to the identification of binding sites for manycellular transcription factors, some of which seem to be crucialfor tissue and disease specificity and tumorigenicity (11, 32,46, 59, 60, 75). One striking example is the core bindingfactor: first identified as a factor binding to the core motifpresent in simian virus 40, polyomavirus, and MuLV enhancers (72),this transcription factor is now involved in the regulation ofa growing number of genes specifically expressed in lymphoid ormyeloid lineages (28, 49, 55, 63, 71, 78, 79). Thecore motif was shown to play a key role in disease specificityfor several MuLV (11, 59). Other cellular factors playinga role in viral gene regulation are ETS family members (62),CAAT/enhancer binding proteins, AP1, NF1, helix-loop-helix (HLH)proteins binding to E-boxes, Oct proteins, and hormone receptors(14, 38, 47). Thus, analysis of retroviral regulatory regionscan lead to new insights into the control of gene expression ineucaryotes.

We have undertaken an analysis of the factors binding to the U3 region of two murine retroviruses that induce myeloid leukemia:Cas-Br-E and Graffi leukemia virus.

Cas-Br-E induces a wide variety of hematopoietic tumors in NFS/N mice; however, injection in NIH Swiss mice causes mainlya non-T, non-B leukemia composed of blasts lacking any myeloidor lymphoid markers (13, 54). Genetic analyses have shownthat the determinants for leukemogenicity are dispersed in differentregions of the genome, including the LTRs (36). We have shownthat the virus preferentially targets two potential oncogenes,fli-1 and evi-1, in 70 and 18% of the tumors, respectively (5-7).

We have recently molecularly cloned the Graffi MuLV and shown that the molecular clones induced the same pathologic responsesin BALB/c and NFS mice as the parental mixture did, i.e., a granulocyticleukemia, composed of myeloblasts and neutrophils with characteristicdonut-like nuclei (54, 56). Two molecular clones, GV1.2 andGV1.4, have been characterized and shown to cause the same disease.They were highly similar, except for the presence of a perfect60-bp duplication in the U3 region of the GV1.2 clone, which displaysa shorter latency period. This correlation between the latencyperiod and the number of enhancer repeats strongly suggest a rolefor the U3 region in the leukemogenic potential and disease specificity.

Two of the regions found protected by DNase I footprinting analyses contain potential binding sites for GATA factors (1a).GATA factors are a family of DNA binding proteins that recognizethe motif (A/T)GATA(A/G) (24, 44, 51). They possess a zincfinger of the form Cys-X₂-Cys-X₁₇-Cys-X₂-Cys (24, 65). Thefounding member, GATA-1, was identified as a positive regulatorof globin gene transcription (23) and has since been involvedin the regulation of all known erythroid specific genes (50,74). At least six GATA family members have been identified:GATA-1, GATA-2, and GATA-3 are involved in the regulation of hematopoiesis-specificgenes (reviewed in reference 50) and are required for normalhematopoietic development in mice (51, 66, 74). Given thiscrucial role of GATA family members in hematopoietic gene regulation,one would not be surprised if they were involved in the transcriptionregulation of leukemia viruses.

Here, we identify in the Cas-Br-E and Graffi U3 regions two GATA elements and show that GATA-1, GATA-2, and GATA-3 can bindto these elements. We also demonstrate that those three familymembers can indeed transactivate Cas-Br-E and Graffi LTR-drivenexpression.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cell lines and nuclear extracts. Myeloid cell-derived M1, M-NFS-60, WEHI-3B, and 32Dcl3 cell lines, T-cell lines Ti-6, BW5147, EL4, and Jurkat, and the B-cellline A20 were maintained in RPMI 1640 medium supplemented with10% fetal calf serum, and 5% WEHI-3B conditioned medium was addedas a source of interleukin-3 for the M-NFS-60 and 32Dcl3 celllines. Erythroid cell lines D1B, MEL, and CB7 were cultured inEagle minimum essential medium supplemented with 10% fetal calfserum, and NIH 3T3, CHO, and COS-7 cells were cultured in Dulbeccomodified Eagle medium plus 10% calf serum.

Nuclear extracts were prepared from 10⁹ cells as described by Wall et al. (70). The protein concentration in the extractswas between 5 and 15 µg/ml. Microextracts were prepared from 10⁶ to 10⁷ cells as described by Andrews and Faller (1). Extracts werealiquoted and stored at $-$ 80°C.

Oligonucleotides. Oligonucleotides were synthesized on a Gene Assembler Plus apparatus (Pharmacia) by the deoxyphosphoamidite method. Theirsequence is shown in Fig. 1.

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FIG. 1. Schematic diagram of a retroviral LTR showing the region analyzed in this study. Sequences from a portion of the Cas-Br-E and GV1.4 U3 regions are compared. Asterisks show differences between Cas-Br-E and Graffi sequences. The sequence of synthetic oligonucleotides C4, G4, and CG5 used in EMSA is underlined. Nucleotides are numbered from the 5' end of U3. Conserved binding sites for other transcription factors (CBF, LVb, NF1, and E-box) are indicated.

Protein-DNA interaction analyses. (i) Electrophoretic mobility shift assays (EMSA). A 50-ng portion of sense oligonucleotide was 5'-end labeled with T4 polynucleotide kinase and [ $gamma$ -³²P]ATP and annealed with 200 ng of the complementary oligonucleotide.A 10-µg portion of nuclear extract was added to 0.8 ng of thelabeled double-stranded oligonucleotide in 10 mM HEPES (pH 7.9)containing 4% glycerol, 1% Ficoll, 200 µg of poly(dI-dC) per ml,25 mM KCl, 1 mM dithiothreitol, 0.5 mM EDTA, and 25 mM NaCl (totalvolume, 10 µl). After a 20-min incubation at room temperature,1 µl of a 20% Ficoll-0.2% bromophenol blue-0.2% xylene cyanolsolution was added and the samples were run on a 4% acrylamidenondenaturing gel in 0.5× Tris-borate-EDTA (TBE) at 150 V for90 min. The dried gels were autoradiographed on Kodak X-Omat films.For competition assays, a 100-fold excess (80 ng) of cold double-strandedoligonucleotide was added before addition of the nuclear extract.For supershift assays, nuclear extracts were incubated with 1to 2 µl of antibodies for 30 min at 0°C.

(ii) Methylation interference. A 50-ng portion of 5'-end-labeled oligonucleotide (upper or lower strand) was partially methylated with dimethyl sulfate asdescribed previously (57). After two ethanol precipitations,the oligonucleotide was annealed with 200 ng of the complementaryoligonucleotide. About 3 × 10⁵ cpm of oligonucleotide was subjected to EMSA as described above,except that the reaction mixture was scaled up threefold. Thewet gel was autoradiographed, and the free and bound oligonucleotideswere eluted separately in 300 µl of elution buffer, extractedwith phenol-chloroform, and ethanol precipitated. The recoveredoligonucleotides were then cleaved by piperidine treatment, andanalyzed on a 10% acrylamide sequencing gel.

Plasmid construction. Standard methods (57) were used in all plasmid constructions.

LTR-chloramphenicol acetyltransferase (CAT) plasmids are derived from pSV0CAT, donated by C. Gorman (27). To construct pCasCAT,the XbaI-PstI fragment from a permuted molecular clone of Cas-Br-E(53), containing two LTRs, was inserted in the HindIII siteof pSV0CAT with HindIII linkers. One LTR was then removed by KpnIdigestion followed by self-ligation. The resulting plasmid contains465 nucleotides of the envelope gene, the entire LTR, and about100 nucleotides of the gag gene, located upstream from the bacterialCAT gene. The others constructions were derived from pCasCAT,by exchanging the HindIII-KpnI (Env-U3) fragment with a 0.6-kbpRsaI-KpnI fragment from Graffi clone GV1.2 (56) to generatepGV1.2CAT and with a 0.9-kbp RsaI-KpnI fragment from Graffi cloneGV1.4 (56) to generate pGV1.4CAT.

Simian virus 40-GATA-1 was constructed by inserting a SalI-XbaI fragment containing the GATA-1 coding sequence into the pSV2vector (27). pMT2 and pMT2-GATA-2, in which the human GATA-2cDNA is expressed from the adenovirus major late promoter, wereobtained from S. Orkin (22). Mouse GATA-3 expression vectorsconsisting of GATA-3 cDNA in the sense or antisense orientationunder the control of Rous sarcoma virus LTR were obtained fromJ. Engel.

Transient-transfection assays. COS-7 cells were transfected with DEAE-dextran, using a 10% dimethyl sulfoxide shock with 2.5 µg of LTR-CAT plasmid and 0to 7.5 µg of GATA expression vector (made up to 7.5 µg with theempty vector when necessary). At 48 h after transfection, thecells were washed in cold phosphate-buffered saline and whole-cellextracts were prepared by three freeze-thaw cycles in 0.25 M Tris-HCl(pH 7.8). Cell extracts were clarified by a 5-min centrifugationat 10,000 × g. The protein concentration was assessed by the Bradfordmethod (Bio-Rad), and equal amounts of total protein were usedfor the determination of CAT activity. CAT activity was measuredby using [¹⁴C]acetyl coenzyme A and extraction with organic solvents as describedpreviously (57). The results were expressed as the amount ofradioactivity present in the organic phase, from which was subtractedthe result obtained with mock-transfected cells (or cells transfectedwith pSV0CAT). We chose not to use a cotransfected expressionvector, like Rous sarcoma virus- $beta$ -galactosidase to monitor transfectionefficiency, because we have shown that it can lead to experimentalbias, since the $beta$ -gal expression level can be influenced by thepresence of other plasmids (8). Instead, we performed eachexperiment several times, at least in triplicate.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

A distinct CG5 binding factor is present in erythroid, myeloid, and lymphoid cell extracts. A previous analysis of the factors binding to Cas-Br-E and Graffi U3 regions by footprinting and EMSA has demonstrated theexistence of an abundant, hematopoietic cell-specific factor,binding to a very well conserved, central part of U3 (200 bp fromthe 5' end [Fig. 1]) (1a). We have attempted to identify thisfactor.

The sequence found protected in footprint analyses is present in Cas-Br-E and Graffi clone 1.4 in this region, and so onedouble-stranded oligonucleotide (CG5) spanning the entire protectedregion was used to study DNA-protein interactions. EMSA performedwith nuclear extracts from several hematopoietic cell lines revealedone strong retarded band (Fig. 2). This signal was competed bya 100-fold excess of cold CG5 oligonucleotide but not by a nonspecificoligonucleotide demonstrating the specificity of the binding (Fig.2, lanes 2 to 13). Interestingly, a slight difference in migrationwas observed with extracts from different hematopoietic cell types:the complex formed with all myeloid cell extracts had a slowermigration than with T-lymphoid cell extracts (lanes 15 to 17),and erythroid cell extracts showed a even faster-migrating complex(lane 14). This observation was confirmed by analysis of othermyeloid (32Dcl3), lymphoid (BW5147 and EL4), and erythroid (D1Band CB7) cell lines (data not shown). These results suggest thatCG5 oligonucleotide can form different complexes, each specificfor myeloid, erythroid, and lymphoid cell types. These complexescould be formed either by distinct proteins binding to the samesequence or by the same protein bearing different posttranslationalmodifications that can alter its mobility.

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FIG. 2. Analysis of the CG5 binding factors by EMSA. End-labeled oligonucleotide CG5 was incubated with nuclear extracts (N.E.) from the following cell lines: MEL (lanes 2 to 4 and 14), Ti-6 (lanes 5 to 7 and 14), M-NFS-60 (lanes 8 to 10 and 16), and M1 (lanes 11 to 13 and 17). Competition (Comp.) was performed with a 100-fold excess of cold CG5 (lanes 3, 6, 9, and 12) or nonspecific (NS) oligonucleotide (lanes 4, 7, 10, 13). Lane 1 contained no nuclear extract.

Methylation interference analysis indicates a contact with two putative GATA binding sites. To gain more information about the precise sequence recognized by the CG5 binding factor(s), methylation interference analyseswere performed with myeloid (M-NFS), erythroid (D1B), and lymphoid(Ti-6) cell extracts. The results (Fig. 3) show similar interferencepatterns with the three nuclear extracts and indicate that oneor more factors make a strong contact with two G residues (positions10 and 21 from the 5' end) on the upper strand and a weaker contactwith G24 on the lower strand. These nucleotides are part of twopotential binding sites for members of the GATA family. Thus,the factors present in myeloid, lymphoid, and erythroid cellsrecognize exactly the same sequence, consisting of two imperfectGATA sites.

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FIG. 3. Methylation interference analysis of the CG5 binding factors. The analysis was performed on the CG5 probe labeled on either the upper (coding) or lower (noncoding) strand, with M-NFS-60, Ti-6, or D1B nuclear extract. C, control (oligonucleotide not incubated with nuclear extract); F, free probe; B, probe recovered from the DNA-complex band. The sequence of the double-stranded oligonucleotide is shown below. Residues whose methylation interferes partially or totally with the binding are indicated by open and solid circles, respectively. Potential GATA sites are underlined.

CG5 binding factors are members of the GATA family. Although the identified GATA sites do not match perfectly with the consensus sequence WGATAR (44), we hypothesized thatthe CG5 binding factors could be different members of the GATAfamily, which would be consistent with the variation observedin their mobility. GATA-1 was likely to be found in erythroidcells, whereas myeloid and T-lymphoid cell types could containGATA-2 and GATA-3, respectively.

Indeed, supershift assays with anti-GATA-1 antibodies showed a supershift of the erythroid cell-specific complex only (Fig.4A, lanes 2 and 4). This identification of the erythroid cell-specificCG5 binding factor as GATA-1 was confirmed by transfecting a GATA-1expression vector in CHO cells: EMSA performed with extracts fromGATA-1-transfected but not mock-transfected CHO cells showed acomplex similar to that obtained with D1B nuclear extracts (Fig.4A, lanes 5 and 6). Similarly, the signal observed with myeloidcell extracts could be supershifted by an anti-GATA-2 antiserumbut not by a preimmune serum (Fig. 4B, lanes 1 to 7); furthermore,nuclear extracts of COS-7 cells transfected with a GATA-2-expressingplasmid elicited a very similar signal, which could also be supershiftedby anti-GATA-2 antibodies (Fig. 4B, lanes 8 to 11). Lastly, thecomplex elicited by T-cell extracts contains GATA-3, since itcould be supershifted only by anti-GATA-3 antibodies (Fig. 4C).No cross-reaction was observed between the anti-GATA-1, anti-GATA-2,and anti-GATA-3 antisera, confirming our identification of threedifferent GATA family members binding to the same sequence (datanot shown).

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FIG. 4. Identification of the CG5 binding factor. (A) GATA-1. EMSA was performed with labeled CG5 and nuclear extracts (N.E.) from CB7 (lanes 1 and 2), D1B (lanes 3 and 4), or CHO transfected with vector pSV2 (lane 5) or with pSV2 GATA-1 (lane 6). Supershift assays were performed with an anti GATA-1 antiserum (lanes 2 and 4). The supershift is indicated by an arrow. (B) GATA-2. CG5 was incubated with the following cell extracts: M-NFS-60 (lanes 2 to 4), M1 (lanes 5 to 7), or COS-7 transfected with vector pMT2 (lane 8) or with pMT2-GATA-2 (lanes 9 to 11). Supershift assays were performed with a preimmune serum (p) (lanes 3, 6, and 10) or an anti-GATA-2 antiserum (G2) (lanes 4, 7, and 11). (C) GATA-3. CG5 was incubated with Ti-6 nuclear extracts and a preimmune serum (p) (lane 2) or an anti-GATA-3 antiserum (G3) (lane 3). (D) GATA factors bind preferentially to the more distal GATA motif. Oligonucleotides bearing mutations destroying the proximal (Mut G1) or distal (Mut G2) GATA sites were used in EMSA with D1B nuclear extracts. Supershift assays were performed with an anti-GATA-1 antiserum. The position of the GATA-1-containing complex is shown, and supershift is indicated by an arrow. The sequence of mutated oligonucleotides is shown below.

EMSA performed with 32Dcl3 cell extracts showed the presence of two specific retarded bands with mobilities similar to thoseof GATA-1 and GATA-2. The 32Dcl3 cell line is a very immaturemyeloid cell line, which can be induced to differentiate alongthe erythroid, monocytic, or granulocytic lineage by using variousdifferentiation-inducing agents (68). These cells were shownto express both GATA-1 and GATA-2 in their undifferentiated stage,as a lot of immature progenitors do (18, 45). Supershift assaysconfirmed the presence of both GATA-1- and GATA-2-containing complexes(data not shown). The GATA-1 signal was always stronger, suggestingeither the presence of more GATA-1 in these cells or a betteraffinity of this family member for the GATA elements in oligonucleotideCG5.

The presence of only one retarded band in EMSA suggests that GATA factors bind only one of the two GATA elements present inoligonucleotide CG5 at a time, even if the two sites were foundoccupied in methylation interference analysis. This could be dueto steric hindrance or to a much higher affinity of GATA factorsfor one of the two sites. To determine which of the two GATA motifswas preferentially used, mutations destroying either the proximal(mutG1) or distal (mutG2) GATA element were introduced into oligonucleotideCG5. EMSA and supershift assays performed with these mutated oligonucleotidesand D1B nuclear extracts show that destroying the proximal elementdoes not impair the binding of GATA-1, but it is abolished ifthe distal element is destroyed (Fig. 4D). However, the proximalelement must participate in the observed complex, since oligonucleotidemutG1 does not compete as well as the wild-type CG5 for GATA-1binding (data not shown). Essentially the same results were obtainedwith extracts from myeloid and T-lymphoid cell lines (data notshown), suggesting that GATA-2 and GATA-3 also have a better affinityfor the second GATA element.

GATA-1 binds at least another site in the Cas-Br-E and Graffi U3 regions. The finding that GATA factors can bind to at least two sites in Cas-Br-E and Graffi U3 regions prompted us to look for otherGATA elements, especially in regions found protected by DNaseI footprinting (1a). Indeed we identified two other putativeGATA sites: one at the 5' end of the LTR (CCATC, nucleotides 14to 18), present only in Cas-Br-E LTR, and one next to the core,shared by the two retroviruses (GGATAT [Fig. 1]). Supershift assaysfailed to identify any GATA-related factor binding to the 5'-endsite (data not shown). On the other hand, oligonucleotides C4and G4, representing nucleotides 135 to 160 in Cas-Br-E and 132to 157 in GV1.4, respectively (Fig. 1), were shown upon EMSA analysisto bind not only the core binding factor (CBF $alpha$ / $beta$ ), present inmyeloid and lymphoid cell extracts, but also an erythroid cell-specificfactor. This erythroid cell-specific complex was not dependenton an intact core element, suggesting the presence of anotherbinding site in that region (1a). Antibodies against GATA-1were able to supershift the complex formed with oligonucleotideC4 or G4, although not to the same extent as with oligonucleotideCG5 (Fig. 5, lane 3). Furthermore, when extracts from CHO cellstransfected with a GATA-1 expression construct were used in EMSA,a complex similar to the erythroid cell-specific complex was observed(Fig. 5, lanes 4 and 5). Thus, GATA-1 is able to bind the GATAelement located near the core but is probably not the only factorresponsible for the complex observed with erythroid cell extracts.Antibodies against GATA-2 or GATA-3 failed to show any supershiftwith erythroid, myeloid, or lymphoid cell extracts.

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FIG. 5. GATA-1 also binds to region IV. EMSA was performed with oligonucleotide C4 and extracts from the following cell lines: D1B (lanes 2 and 3), CHO (lane 4), and CHO transfected with the pSV2 GATA-1 (lane 5). Lane 1, no nuclear extract. Lane 3 shows the supershift assay with an anti-GATA-1 antiserum. The supershift is indicated by an arrow.

GATA factors are able to transactivate expression from Cas-Br-E and Graffi LTRs. As in any retroviruses, cis-acting elements important for Cas-Br-E and Graffi transcription regulation are likely to be locatedin the U3 region of the LTR. Since GATA factors are able to bindto more than one site in this region, we were interested in whetherthey could influence transcription driven from Cas-Br-E and Graffipromoter-enhancer regions. To this end, the entire Cas-Br-E LTRwas cloned upstream from the bacterial CAT gene. From this LTR-CATconstruct, the Cas-Br-E U3 region was removed and replaced bythe same fragment from Graffi LV clone GV1.2 or GV1.4. Each ofthose three reporter plasmids was cotransfected in COS-7 cells,with expression vectors carrying GATA-1, GATA-2, or GATA-3 codingsequence, and CAT activity was measured 48 h posttransfection.These transient-transfection assays were repeated several timesin triplicate, and representative results are shown in Fig. 6.

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FIG. 6. LTR transactivation by GATA factors. LTR-CAT constructs containing Cas-Br-E, GV1.2, or GV1.4 U3 regions were cotransfected with GATA-expressing vectors in COS-7 cells as described in Materials and Methods. CAT activity was measured and compared with the activity observed with an empty expression vector, which was given the arbitrary value of 1. The mean values and standard deviations for a typical triplicate experiment are shown. (A) GATA-1. The LTR-CAT plasmid (2.5 µg) was cotransfected with 0, 2.5, 5, or 7.5 µg of pSV2 GATA-1. The total amount of expression vector was completed to 7.5 µg with the empty vector pSV2. (B) GATA-2. The LTR-CAT plasmid (2.5 µg) was cotransfected with 5 µg of the empty vector pMT2 or 5 µg of pMT2 GATA-2. (C) GATA-3. The LTR-CAT plasmid (2.5 µg) was cotransfected with 5 µg of pRSV GATA-3 in the sense or antisense orientation.

These results suggest that GATA-1 is able to transactivate Cas-Br-E, GV1.2, and GV1.4 LTRs in a dose-dependent fashion witha maximum at 5 µg of expression vector for 2.5 µg of reporterplasmid. At this ratio, Cas-Br-E, GV1.4, and GV1.2 promoter weretransactivated 2-, 2.5-, and 2.8-fold (Fig. 6A). Transactivationwas also observed with GATA-2, varying from 3.6-fold for GV1.4to 5.11-fold for GV1.2 (Fig. 6B). Lastly, cotransfection of aGATA-3 expression vector in the sense orientation led to a 1.5-to 2.5-fold transactivation of the viral LTRs compared to theantisense orientation (Fig. 6C). The transactivation rate variedfrom one experiment to another but was always significant. Thus,these results suggest that three members of the GATA family areable to transactivate Cas-Br-E and Graffi expression. The Grafficlone GV1.2 LTR, which has the strongest activity in COS-7 cells,also showed the greatest transactivation by the three GATA factors.Clone GV1.4 and Cas-Br-E displayed roughly the same transactivationpattern, ranging from 1.5- to 4-fold. The transactivations observedwith GATA-1, GATA-2, and GATA-3 cannot be compared since theirexpression was driven by different promoters.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The goal of this work was to identify some of the factors binding to the promoter-enhancer region of two MuLV, Cas-Br-E andGraffi MuLV. The results presented above indicate that at leastthree members of the GATA family of transcription factors, GATA-1,GATA-2, and GATA-3, are able to bind to three GATA elements andto transactivate LTR-driven expression.

The three GATA motifs identified here do not perfectly match the consensus WGATAR described for GATA binding factors (23,44). However, analyses of the GATA protein binding specificityby PCR-mediated random-site selection have shown binding to sequencesquite different from this consensus: in particular, CGATAT wasshown to bind GATA-1 and GATA-2 and TGATGG could weakly bind GATA-2and GATA-3 (44). Our results indicate that the motifs AGATGGand/or AGAGAT strongly bind GATA-1, GATA-2, and GATA-3 and thatGGATAT binds at least GATA-1.

Two putative GATA elements are present in oligonucleotide CG5 (Fig. 1). Methylation of the G residue in the two elements interfereswith the binding of the factors present in erythroid, myeloid,and T-lymphoid cell extracts (Fig. 3), which were identified asGATA-1, GATA-2, and GATA-3, respectively (Fig. 4). Hence, thetwo GATA elements seem capable of binding each GATA protein; however,only one complex, corresponding to one bound factor, was observedin EMSA, even when large amounts of nuclear extracts were used(data not shown). Moreover, mutations destroying the second siteclearly abolish the complex formation while mutations destroyingthe first site only slightly diminish the affinity of the CG5oligonucleotide for GATA factors, since the mutated oligonucleotidedoes not compete as well as the wild type (Fig. 4D and data notshown). Thus, the more distal motif AGATAT must be responsiblefor the complex observed with oligonucleotide CG5. This resultis surprising since the same motif is present in oligonucleotideC4, which binds GATA factors only poorly. This difference is probablydue to the presence of other sites in oligonucleotide C4, whichmay interfere with the binding of GATA factors. Also, the motifAGATGG is a better match to the consensus sequence for GATA-1and GATA-2, determined by PCR-mediated random-site selection (44).However, this site is overlapping with an E-box motif (CAGATG)named E_GRE, well conserved among MuLV (Fig. 1). A factor bindingto this motif has been identified and named ALF1. This class Abasic HLH (b-HLH) transcription factor has been shown to transactivatethe LTRs of several MLVs including Akv, SL3-3, Moloney MuLV, andspleen focus-forming virus (46). Also, this site is includedin a perfect consensus site (10-of 10-nucleotide match) for theTAL1/SCL transcription factor (33), a class B b-HLH protein(16, 17). The tal-1 gene was found rearranged in 25% of casesof human acute T-cell lymphoblastic leukemia (4, 16), andknockout studies have identified it as a key factor in the regulationof hematopoiesis (10). Although we have not been able to demonstratethe binding of a TAL-related factor by supershift assays, it hasbeen shown that TAL1 indeed can form heterodimers with ALF1 thatbind specifically to this site in the Akv or Moloney MuLV U3 regionand can modulate the transcriptional activation of MuLV by ALF-1(48). Thus, at least three transcription factors can bind tothe same region: GATA factors, ALF-1 homodimers, and TAL-1 inheterodimers with class A b-HLH proteins. Interestingly, TAL1was shown to participate in a large oligomeric complex with E47,GATA-1, Lmo2, and Ldb/NL1, which bind a bipartite DNA motif comprisingan E-box followed 9 bp downstream by a GATA site (69). Thisbipartite motif is reminiscent of the E-box/GATA motif presentin oligonucleotide CG5, although the spacing between the two motifsis different. Thus, tal-1 could interact with GATA-1 and other,unknown factors to form a large transactivating complex.

Another putative GATA site is present in oligonucleotide C4 (Cas-Br-E) or G4 (Graffi). A GATA-related complex was observedonly with erythroid cell nuclear extracts. This complex was slightlysupershifted by anti-GATA-1 antibodies, and extracts from GATA-1-expressingCHO cells gave rise to a complex with identical mobility (Fig.5). These observations indicate that GATA-1 is able to bind tothis site, perhaps with a weak affinity. The anti-GATA-1 antiserumwas not able to supershift the entire band, suggesting that thisretarded band is composed of more than one complex with similarmobilities, one of which contains GATA-1. This GATA element islocated next to the core element and overlaps with an Ets bindingsite (EBS), which is well conserved among MuLV (26). Ets familymembers can bind to the EBS motif (also called LVt) in the MoloneyMuLV enhancer (30, 43) and transactivate LTR-driven expression(62). We have already shown that when myeloid or lymphoid cellextracts are used the complex observed is formed by the heterodimerCBF $alpha$ / $beta$ (1a). Although the EMSA studies were done with an excessof probe, binding of GATA family members seems to be observedonly with extracts containing small amounts of CBF, like erythroidnuclear extracts, and we were unable to show any binding of Etsfamily members. Experimental conditions could be responsible forthese observations. Indeed, the type of gel used in EMSA has beenshown to greatly influence the complex observed: complexes involvingeither CBF or LVt are observed with the Mo-MuLV enhancer, dependingon the buffer used in the gel (43). Possibly, GATA-2- or GATA-3-containingcomplexes would be observed with myeloid and lymphoid cell extractsunder different EMSA conditions. Nevertheless, at least threedifferent transcription factors are able to bind to a region assmall as 15 bp. The exact combination of bound factors is probablydetermined by the availability and relative abundance of eachfactor in the infected cell, their respective affinity, as wellas interactions with adjacent complexes.

Our results demonstrate that the binding of GATA factors may have a functional significance, since they are indeed able toactivate the transcription from the viral promoter (Fig. 6). Thistransactivation, although not very strong (1.6- to 5-fold), wasreproducibly observed with GATA-1, GATA-2, and GATA-3 on the threeviral promoters studied: Cas-Br-E, GV1.2, and GV1.4. A similaractivating potential has been reported for GATA factors: a threefoldactivation was demonstrated for GATA-1 on the platelet glycoproteinIIb (GpIIb) (41) and the SCL (39) gene promoters and for GATA-2on the endothelin-1 promoter (37, 40). This modest effectis easily explained by the fact that a multitude of transcriptionfactors cooperate to activate LTR-driven transcription, so theeffect of one factor is assessed by comparison with an alreadyhigh transcription level due to the presence of other factors.Our data do not allow the evaluation of the effect of each GATAelement on the transactivation. However, the observed transactivationis always stronger for the GV1.2 clone of Graffi virus than forthe GV1.4 clone. The GV1.2 U3 region possess two copies of a 50-bpdirect repeat and hence two copies of the more proximal GATA element;thus, the stronger activation observed indicates that this proximalGATA site might be involved in the activation. Mutagenesis studiesare required to precisely define which GATA elements are usedin vivo.

The three members studied here are essential to the normal development of the hematopoietic system and subsequent hematopoiesis(9, 52, 66, 73). GATA-1 is expressed in all erythroidcell lineages, megakaryocytes, mast cells, and mutipotent stemcells and has been involved in the regulation of most erythroidgenes (45; reference 50 and references therein). GATA-3 isexpressed at all stages of T-cell development (80). GATA-2 hasa much broader expression pattern including all myeloid and erythroidcell lineages and endothelial cells (50), and is essential formultilineage hematopoiesis (67). It is likely to act as a generaltranscription factor (40). It is not surprising that those threekey factors in hematopoiesis should be involved in the transcriptionalregulation of retroviruses that target primarily hematopoieticcells and cause leukemia. Cas-Br-E and Graffi MuLV both inducemyeloid leukemia; therefore, the target cell is most probablya myeloid progenitor which expresses GATA-2 and possibly GATA-1.The GATA elements described here are well conserved in other murineretroviruses that induce erythroleukemia (Friend MuLV) or T-celllymphoma (Moloney MuLV, SL3-3, radiation leukemia virus, etc.)(Fig. 7). In these cases, the target cell for transformation islikely to express GATA-1 or GATA-3, respectively; therefore, transcriptionof these viruses may also be regulated by GATA factors. The differentmembers of the GATA family seem to be highly interchangeable (51);for example, GATA-3 and GATA-4 can compensate for a GATA-1 defect(9). Indeed, our results show that the three members GATA-1,GATA-2, and GATA-3 are able to activate transcription from retroviralpromoters. Hence, GATA factors alone are probably not responsiblefor the tissue and disease specificity of Cas-Br-E, Graffi, orother MuLV. On the contrary, they could ensure a strong expressionin a very broad spectrum of lineages: instead of one ubiquitousfactor, a set of different but very similar factors could be usedin different cell types. One could hypothesize that GATA elementscould participate in tissue specificity by cooperating with morespecific elements. Cooperation of GATA factors with other transcriptionfactors has been described in several cases: GATA-1 cooperateswith Ets to activate the platelet glycoprotein Ib and IIb (GpIband GpIIb) promoters (31, 41) and also with SP1 and EKLF (29);GATA-2 cooperates with the AP-1 complex to activate the endothelin1 promoter (37); cooperation with CREB and with SP1 has alsobeen described (39, 61). In some cases, a direct protein-proteincontact has been demonstrated (29). Such a cooperation couldbe possible between GATA factors and CBF, since the more proximalGATA site is located next to the core motif. CBF is known to actalmost always in cooperation with other transcription factors.A cooperation between CBF and Ets family members to activate theMoloney MuLV enhancer has been demonstrated, with a simultaneousbinding of CBF to the core and an Ets protein to the EBS, whichoverlaps the GATA motif (62). Also, CBF can cooperate with Mybto transactivate the SL3-3 enhancer (77). It is tempting tohypothesize that CBF can cooperate with either Ets factors orGATA factors, depending on the relative amounts of these factorsin the infected cell. However, we did not observe any cooperationbetween GATA and CBF $alpha$ in cotransfection experiments. Moreover,there was no additive effect of GATA over CBF transactivationand vice versa (data not shown). This suggests that either CBFor GATA factors can regulate MuLV transcriptional activity, dependingon their relative abundance in a given cell type.

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FIG. 7. Conservation of GATA binding sites among various MuLV. The sequence of the GATA element in oligonucleotide C4 and the proximal (p) and distal (d) oligonucleotide CG5 are shown. Data from references 26, 54, and 56.

A transactivation of other MuLV by GATA-1 has been reported: in transient transfection in CV-1 cells, GATA-1 was shown totransactivate Friend MuLV and Moloney MuLV LTRs 15- and 4-fold,respectively (15). In COS-7 cells, we observed a more modestfourfold induction of the Friend MuLV LTR by GATA-1 (data notshown), which is comparable to the induction of 2- and 2.8-foldobtained with Cas-Br-E and Graffi, respectively. However, a strongactivation of the Friend MuLV LTR by GATA-1 would not be surprisingsince it possesses additional perfect GATA sites. Since FriendMuLV is a truly erythroid cell-specific virus, it would be interestingto assess its transcriptional activation by other, nonerythroidmembers of the GATA family like GATA-3, to determine if the specificityof this virus for erythroid cell types is related to a specifictranscriptional regulation by GATA-1.

Interestingly, we found that in 70% of tumors induced by Cas-Br-E, the fli-1 gene is activated by a promoter insertion mechanism(5). All the proviruses were found integrated in the same transcriptionalorientation as fli-1, within 30 bp at the end of exon 1 (2,54). We showed recently the presence of a EBS-GATA dual bindingsite in this exon 1 which binds GATA-1 and the Ets family memberSpi1/PU-1, and we hypothesized that Spi1 could negatively regulatefli-1 (3). The integration of Cas-Br-E provirus downstreamof this site bypasses this regulation; however, fli-1 may stillbe regulated by GATA and Ets factors, this time through the LTR,leading to overexpression.

The implication of GATA factors in the transcription regulation of MuLV adds even more complexity to the already complex modelarray of cis-acting elements in the regulatory region and stressesthe importance of interactions between several regulatory elementsto achieve a fine regulation of transcription.

	ACKNOWLEDGMENTS

We thank S. Orkin and J. Engel for providing the mouse GATA-2 and GATA-3 expression vectors, respectively; Richard Bergeronfor excellent technical assistance; and Simon Labelle and EricCarpentier for providing the excellent illustrations. We thankElsy Edouard and Laurent Poliquin for helpful discussions.

We gratefully acknowledge financial support from the National Sciences and Energy Research Council of Canada.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire de biologie moléculaire, Département des Sciences Biologiques, Universitédu Québec à Montréal, C.P. 8888, Succursale Centre-Ville, Montréal,Québec, Canada H3C 3P8. Phone: (514) 987-3000, ext. 3953. Fax:(514) 987-4647. E-mail: rassart.eric{at}UQAM.ca.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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68. Valtieri, M., D. Tweardy, D. Caracciolo, K. Johnson, F. Mavilio, S. Altmann, D. Santoli, and G. Rovera. 1987. Cytokine-dependent granulocytic differentiation. Regulation of proliferative and differentiative responses in a murine progenitor cell line. J. Immunol. 138:3829-3835[Abstract].

69. Wadman, I. A., H. Osada, G. G. Grutz, A. D. Agulnick, H. Westphal, A. Forster, and T. H. Rabbitts. 1997. The LIM-only protein Lmo2 is a bridging molecule assembling an erythroid, DNA-binding complex which includes the TAL1, E47, GATA-1 and Ldb1/NLI proteins. EMBO J. 16:3145-3157[Medline].

70. Wall, L., E. deBoer, and F. Grosveld. 1988. The human beta-globin gene 3' enhancer contains multiple binding sites for an erythroid-specific protein. Genes Dev. 2:1089-1100[Abstract/Free Full Text].

71. Wang, S. W., and N. A. Speck. 1992. Purification of core-binding factor, a protein that binds the conserved core site in murine leukemia virus enhancers. Mol. Cell. Biol. 12:89-102[Abstract/Free Full Text].

72. Weiher, H., M. Konig, and P. Gruss. 1983. Multiple point mutations affecting the simian virus 40 enhancer. Science 219:626-631[Abstract/Free Full Text].

73. Weiss, M. J., and S. H. Orkin. 1995. Transcription factor GATA-1 permits survival and maturation of erythroid precursors by preventing apoptosis. Proc. Natl. Acad. Sci. USA 92:9623-9627[Abstract/Free Full Text].

74. Weiss, M. J., and S. H. Orkin. 1995. GATA transcription factors: key regulators of hematopoiesis. Exp. Hematol. 23:99-107[Medline].

75. Yoshimura, F. K., K. Diem, H. M. Chen, and J. Tupper. 1993. A protein-binding site with dyad symmetry in the long terminal repeat of the MCF13 murine leukemia virus that contributes to transcriptional activity in T lymphocytes. J. Virol. 67:2298-2304[Abstract/Free Full Text].

76. Yuen, P. H., and P. F. Szurek. 1989. The reduced virulence of the thymotropic Moloney murine leukemia virus derivative MoMuLV-TB is mapped to 11 mutations within the U3 region of the long terminal repeat. J. Virol. 63:471-480[Abstract/Free Full Text].

77. Zaiman, A. L., and J. Lenz. 1996. Transcriptional activation of a retrovirus enhancer by CBF (AML1) requires a second factor: evidence for cooperativity with c-Myb. J. Virol. 70:5618-5629[Abstract/Free Full Text].

78. Zhang, D. E., K. Fujioka, C. Hetherington, L. Shapiro, H. M. Chen, A. Look, and D. G. Tenen. 1994. Identification of a region which directs the monocytic activity of the colony-stimulating factor 1 (macrophage colony-stimulating factor) receptor promoter and binds PEBP2/CBF (AML1). Mol. Cell. Biol. 14:8085-8095[Abstract/Free Full Text].

79. Zhang, D. E., C. Hetherington, S. Meyers, K. Rhoades, C. Larson, H. M. Chen, S. W. Hiebert, and D. G. Tenen. 1996. CCAAT enhancer-binding protein (C/EBP) and AML1 (CBF alpha2) synergistically activate the macrophage colony-stimulating factor receptor promoter. Mol. Cell. Biol. 16:1231-1240[Abstract].

80. Zon, L. I., Y. Yamaguchi, K. Yee, E. Albee, A. Kimura, J. Bennet, S. H. Orkin, and S. J. Ackerman. 1993. Expression of mRNA for the GATA-binding proteins in human eosinophils and basophils: potential role in gene transcription. Blood 81:3234-3241[Abstract/Free Full Text].

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