Cell Signaling Switches HOX-PBX Complexes from Repressors to Activators of Transcription Mediated by Histone Deacetylases and Histone Acetyltransferases

doi:10.1128/MCB.20.22.8623-8633.2000

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Molecular and Cellular Biology, November 2000, p. 8623-8633, Vol. 20, No. 22
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Cell Signaling Switches HOX-PBX Complexes from Repressors to Activators of Transcription Mediated by Histone Deacetylases and Histone Acetyltransferases

Maya Saleh,¹^,² Isabel Rambaldi,¹ Xiang-Jiao Yang,³ and Mark S. Featherstone¹^,²^,⁴^,^*

McGill Cancer Centre,¹ Department of Biochemistry,² Molecular Oncology Group, Department of Medicine,³ and Department of Oncology,⁴ McGill University, Montréal, Québec, Canada H3G 1Y6

Received 26 June 2000/Returned for modification 19 July 2000/Accepted 18 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Hoxb1 autoregulatory element comprises three HOX-PBX binding sites. Despite the presence of HOXB1 and PBX1, this enhancerfails to activate reporter gene expression in retinoic acid-treatedP19 cell monolayers. Activation requires cell aggregation in additionto RA. This suggests that HOX-PBX complexes may repress transcriptionunder some conditions. Consistent with this, multimerized HOX-PBXbinding sites repress reporter gene expression in HEK293 cells.We provide a mechanistic basis for repressor function by demonstratingthat a corepressor complex, including histone deacetylases (HDACs)1 and 3, mSIN3B, and N-CoR/SMRT, interacts with PBX1A. We mapa site of interaction with HDAC1 to the PBX1 N terminus and showthat the PBX partner is required for repression by the HOX-PBXcomplex. Treatment with the deacetylase inhibitor trichostatinA not only relieves repression but also converts the HOX-PBX complexto a net activator of transcription. We show that this activationfunction is mediated by the recruitment of the coactivator CREB-bindingprotein by the HOX partner. Interestingly, HOX-PBX complexes areswitched from transcriptional repressors to activators in responseto protein kinase A signaling or cell aggregation. Together, ourresults suggest a model whereby the HOX-PBX complex can act asa repressor or activator of transcription via association withcorepressors and coactivators. The model implies that cell signalingis a direct determinant of HOX-PBX function in the patterningof the animalembryo.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

HOX proteins are sequence-specific DNA-binding transcription factors that play a crucial role in the specification of anteroposterioridentity in the animal embryo (20, 54). Conservation withinthe DNA-binding homeodomains results in different HOX proteinsrecognizing similar regulatory elements with only modest preferences(reviewed in reference 27). High-affinity DNA binding is achievedwhen HOX proteins are heterodimerized with partners of the PBCfamily (mammalian PBX, Drosophila Extradenticle [EXD], and Caenorhabditiselegans CEH-20) (55). Mammalian MEIS1 has been shown to independentlydimerize with HOX proteins and with PBX (11, 57, 78). Recently,trimeric complexes encompassing all three homeoproteins, HOX-PBX-MEIS,have also been characterized (77, 79). The MEIS-related proteinPREP1, also known as PKNOX1, can additionally form a dimer withPBX, as well as a trimeric complex with HOX and PBX partners (6,7, 15, 34). While the majority of HOX monomers recognizea DNA core motif of TAAT (23), HOX-PBX, HOX-MEIS, and PBX-MEISheterodimers recognize larger motifs resulting in a higher affinityand specificity of DNA binding by these homeoproteins (49).

A conserved motif with the consensus YPWM is found N terminal to the homeodomain of HOX proteins from paralogous groups 1to 8. The YPWM motif contacts the PBX homeodomain and is strictlyrequired for cooperative DNA binding by PBX and HOX partners (49,50). A conserved W in HOX proteins from groups 9 and 10 performsa similar function (12).

The downstream targets of mammalian HOX proteins have been poorly characterized. The best-characterized targets are some Hoxgenes known to be positively autoregulated by their own productsor cross-regulated by the products of other Hox genes (26, 68,69). In these instances, HOX-PBX complexes act as activatorsof transcription. For example, the Hoxb1 autoregulatory element(ARE) contains three binding sites for HOX-PBX complexes. Thesesites are required to direct expression of a Hoxb1 transgene inrhombomere 4 (r4) of the developing hindbrain (68).

Genetic and molecular studies have provided evidence supporting a negative regulatory role for HOX proteins (43). In thecase of decapentaplegic (dpp) regulation in Drosophila, repressionby HOX proteins dominates over activation (9). This impliesactive transcriptional repression by HOX proteins (9, 25,46). In addition, in vitro mapping studies have characterizedrepression domains in different HOX proteins, as well as in thePBX partner (13, 45, 75). Therefore, HOX proteins may beactivators or repressors in a context-dependentmanner.

By analogy to nuclear receptors, HOX-PBX complexes are likely to achieve transcriptional repression or activation throughdifferential association with coactivators and corepressors (81).One class of coregulators are the histone acetyltransferases (HATs)and the histone deacetylases (HDACs), which modify chromatin aswell as nonhistone proteins. The HATs include GCN5, PCAF, CREB-bindingprotein (CBP)/p300, the steroid receptor coactivator class, andthe MYST family (80). On the other hand, the known HDACs includeHDAC1 through -8, with class I HDACs consisting of HDAC1, HDAC2,HDAC3, and HDAC8 (homologues of the yeast RPD3 protein) and classII HDACs consisting of HDAC4, HDAC5, HDAC6, and HDAC7 (homologuesof the yeast HDA1 protein) (for a review, see reference 37).HDAC1 and HDAC2 form the catalytic subunits of two characterizedmultiprotein complexes, the mSIN3A and Mi2 complexes (35). Additionally,HDAC3 has been shown to interact with the corepressor SMRT (28).Recent genetic evidence in C. elegans shows EGL-27, a homologueof MTA1 (a component of the Mi2-HDAC1 complex), in the same pathwayas MAb-5 (86, 94), further implying that HOX proteins mayinteract with HDACs and other histone-modifying enzymes to accomplishtheir developmentalprogram.

In this report, we present evidence for an interaction between HOX-PBX complexes and histone-modifying enzymes and show thatthe activity of the HOX-PBX heterodimer is determined by a regulatedbalance between a corepressor complex consisting of class I HDACs,mSIN3B, and N-CoR/SMRT and a coactivator complex containing CBP.We show, moreover, that activation of the protein kinase A (PKA)signaling pathway significantly potentiates the CBP-mediated transactivationby HOX-PBX complexes. We propose a model in which PKA acts asa signaling switch that converts HOX-PBX complexes from transcriptionalrepressors toactivators.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture and transfections. P19 mouse embryonal carcinoma (EC) cells and human embryonic kidney HEK293 cells were cultured in alpha minimal essentialmedium supplemented with 10% fetal calf serum. Some experimentsemployed 293 T cells constitutively expressing the simian virus40 large T antigen. Transient transfections were performed usingthe calcium phosphate precipitation method as described earlier(72). A lacZ reporter driven by the cytomegalovirus (CMV) enhancerwas used to control for transfection efficiency in some experiments.Because the activity of the CMV enhancer appeared to change inresponse to PKA, a lacZ reporter driven by the Rous sarcoma viruslong terminal repeat was used in transfections involving PKA.For stable transfections of P19, the cells were seeded at a densityof 10⁵ cells/10-cm plate and transfected with a total of 15 µg of DNAconsisting of 9 µg of the transgene of interest (p1230 or b1-ARE-lacZ),1 µg of PGK-puromycin, and 5 µg of pCAB-B17 as the carrier DNA(53). At 40 h posttransfection, cells were selected with 2 µgof puromycin per ml for at least 10 days. Cells were kept in monolayeror aggregated in bacterial petri dishes for 24 h in the presenceor absence of treatment and then reattached in tissue cultureplates overnight (73). The treatment consisted of either retinoicacid (RA) (3 × 10⁷ M) or trichostatin A (TSA; concentrations ranging from 20 nMto 2 µM) or a combination of both RA and TSA. Significant celldeath sometimes occurred in response to TSA; however, this wasvariable and dependent on drug concentration and cell context.HEK293 cells were more sensitive than P19 to TSA-induced celldeath. Cells were treated with the estrogen antagonist $alpha$ -hydroxytamoxifen(TOT) overnight at 10⁷M.

Antibodies. Rabbit polyclonal antibodies raised against PBX1, mSIN3A, or mSIN3B were purchased from Santa Cruz. Rabbit polyclonal antibodiesagainst human HDAC1 and HDAC3 were from Upstate Biotechnology.Rabbit polyclonal antibodies against HOXB1 were generously suppliedby C. Largman. Mouse monoclonal antibodies against the GAL4 DNA-bindingdomain (DBD) (RK5C1), the hemagglutinin epitope (HA-11), and theflag epitope (M2) were purchased from Santa Cruz, Babco, and Sigma,respectively. Mouse monoclonal antibodies were recognized withhorseradish peroxidase (HRP)-conjugated goat anti-mouse ( $kappa$ lightchain) secondary antibodies from PharMingen, and rabbit polyclonalantibodies were recognized by HRP-conjugated protein A-Sepharose(Amersham).

Plasmids. p1230 (generous gift of R. Krumlauf) is a lacZ reporter under the control of the minimal promoter of the $beta$ globin gene. b1-ARE-lacZconsists of the ARE of the Hoxb1 gene (68) cloned by PCR amplificationinto the HindIII-XhoI sites of p1230. pML, pML(5xHOX-PBX), pML5xHOX,and pML5xUAS are luciferase reporters containing the adenovirusmajor late promoter alone, driven by 5xHOX-PBX binding sites (TGATTGAT),5xHOX binding sites (TAAT), or 5xGAL4 binding sites, respectively(67, 72, 77). Expression plasmids for HOXA1, HOXD4, PBX1A,and PBX1A deletion mutants have been previously described (66,77). The HOXB1 expression vector is driven by the beta-actinpromoter. 89-172-HA was constructed by PCR amplification of theregion encoding residues 89 to 172, followed by cloning of theproduct in frame with three copies of the HA epitope in the plasmidpRC/CMV (Invitrogen). Flag-HDAC1, flag-HDAC3 and E1A are describedelsewhere (87, 88, 91) and were generously provided by A.Lai (McGill University). Flag-HDAC4 and flag-PCAF are describedelsewhere (84, 89). Flag-N-CoR, flag-SMRT, HA-CBP, and theCBP domains were generously provided by V. Giguère and A. Tremblay(McGill University, Université de Montréal). GAL4-HOXD4N fusesthe first 141 residues of HOXD4 to the GAL4 DBD and was describedpreviously (72). HOXD4 residues 139 to 250 were fused to theGAL4 DBD to generate GAL4-HOXD4C. An expression vector for thehuman estrogen receptor alpha driven by the CMV enhancer was generouslyprovided by Vincent Giguère (McGillUniversity).

$beta$ -Galactosidase and luciferase assays. Luciferase assays and liquid $beta$ -galactosidase assays were performed as described previously (67). $beta$ -Galactosidase plate assayswere performed after fixation of the cells with a solution of2% formaldehyde-0.2% glutaraldehyde in phosphate-buffered saline(PBS) for 5 min at 4°C. The cells were washed with PBS for threetimes and then stained at 37°C with a solution composed of 5 mMferrocyanide, 5 mM ferricyanide, 1 mg of X-Gal (5-bromo-4-chloro-3-indolyl- $beta$ -D-galactopyranoside)/ml,and 2 mM MgCl₂ inPBS.

Immunoprecipitation assays. At 40 h posttransfection, the cells were harvested and lysed on ice for 30 min with 500 µl of a low-stringency buffer containing150 mM KCl. Whole-cell extracts were precleared with protein A-or protein G-Sepharose (depending on the source of the primaryantibody used) for 30 min. Precleared lysates were incubated with0.5 to 2 µg of primary antibody for 2 h, followed by the additionof 20 µl of a 50% slurry of protein A- or protein G-Sepharosefor 2 to 18 h. Precipitates were washed six times with the lysisbuffer and eluted by boiling in 2× sample buffer for 15 min. Elutedproteins were resolved by sodium dodecyl sulfate-polyacrylamidegel electrophoresis and analyzed after Western blotting to polyvinylidenedifluoride membranes (Millipore). Secondary antibodies used inWestern analysis were HRP conjugated and were detected by enhancedchemiluminescence (NEN Life Sciences). To immunoprecipitate flag-epitope-taggedproteins, a similar protocol was used except that M2 beads (Sigma)were used instead of protein G-Sepharose, and flag peptides (Sigma)were used to elute the precipitated proteins prior toboiling.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

TSA relieves the transcriptional repression of HOX-PBX-responsive enhancers. The induction of Hoxb1 upon RA treatment of mouse embryos is mediated directly by a 3' RA response element (RARE) (51) andindirectly by an ARE (68). The Hoxb1 ARE consists of three cooperativebinding sites for HOX-PBX heterodimers (Fig. 1A, top panel). Twoparalog group 1 HOX proteins, HOXB1 (18) and HOXA1 (M. Phelanand M. S. Featherstone, unpublished observations), can activatetranscription through the Hoxb1 ARE. Both gain- and loss-of-functionexperiments show that HOXA1 and HOXB1 regulate Hoxb1 expressionin the embryonic hindbrain (5, 68, 82, 93). These effectsare very likely to be mediated by the Hoxb1 ARE, as has been demonstratedin one case (68). In addition to HOXB1 and PBX, coexpressionof PREP1 stimulates reporter gene expression through the Hoxb1ARE in transfected cells (6). Together, these results suggestthat the presence of first group HOX proteins, PBX, and membersof the MEIS/PREP family would be sufficient to activate transcriptionthrough the Hoxb1 ARE.

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FIG. 1. TSA relieves the transcriptional repression of HOX-PBX-responsive enhancers. (A) The upper panel schematically represents the b1-ARE-lacZ reporter used to stably transfect P19 cells. The black boxes r1, r2, and r3 represent three previously characterized HOX-PBX binding sites (71). The gray box b1 denotes block 1, a region of homology conserved across species. Ovals labeled "P" and "H" denote the PBX-HOX complex. In the lower panel, a stably transfected transgene containing the Hoxb1 ARE (b1-ARE-lacZ) was active in RA (3 × 10⁷ M)-treated P19 cells only if the cells were aggregated during RA exposure for 24 h (panel d) but not if the cells were kept cultured in monolayers (panel b). P19 cell monolayers are shown in panels a and b, while cell aggregates are shown in panels c and d. The cells in panels b and d were treated with RA at 3 × 10⁷ M for 24 h. (B) TSA induces the activity of the b1-ARE-lacZ in monolayers in the presence or absence of RA. Liquid $beta$ -galactosidase assays were carried out on P19 cells stably transfected with the b1-ARE-lacZ and cultured in monolayer. Monolayers were treated with either RA (3 × 10⁷ M), TSA (20 nM to 2 µM), or a combination of both for 24 h. In the inset, similar assays were performed using a control transgene lacking the Hoxb1 ARE (p1230). (C) HOXB1 and PBX1 are induced in P19 cell monolayers in response to RA or TSA. Western analysis was performed using whole-cell extracts from P19 cells cultured in monolayers in the absence or presence of treatment. RA was used at 3 × 10⁷ M or 10⁵ M, and TSA was at 3 µM.

P19 EC cells differentiate along the neural pathway when aggregated in the presence of RA (73). While RA-treated P19 cellmonolayers fail to form neurons and glia, the products of theHoxb1, Hoxa1, Pbx, Meis, and Prep genes are induced (21, 36,40, 62). We therefore expected that a stable integrated transgenecarrying the Hoxb1 ARE driving lacZ (b1-ARE-lacZ) would be activein RA-treated P19 cell monolayers. Surprisingly, b1-ARE-lacZ waspoorly active in P19 EC cells when cultured in monolayers in thepresence of RA (Fig. 1Ab). The transgene was efficiently activatedonly when RA-treated cells were also aggregated (Fig. 1Ad), suggestingthat cell aggregation provides a signal required for HOXB1-PBXcomplexes to activatetranscription.

An alternative explanation for these results is that the site of integration imposed constraints on the activity of the Hoxb1ARE. However, these experiments were done on populations of multipleclones representing many different sites of integration. Anotherpossibility is that HOXB1, PBX, and MEIS/PREP proteins unexpectedlyfailed to accumulate upon RA treatment. This was not the case,as revealed by Western blot analysis (Fig. 1C). HOXB1 and PBX1were both detected in P19 cell monolayers treated with RA at eitherof two concentrations. HOXB1 showed the most dramatic induction,while PBX1 was already present in untreated cells and was modestlyinduced upon RA treatment. MEIS1 was also present before and afterRA treatment (data notshown).

We hypothesized that in the absence of cell aggregation, HOXB1-PBX complexes could recruit HDACs to the Hoxb1 ARE, therebyestablishing a transcriptionally inactive condensed chromatin.To test this hypothesis, we treated the cells in monolayer withTSA, an HDAC inhibitor, and measured the reporter activity (Fig.1B). As little as 20 nM TSA induced lacZ expression directed bythe Hoxb1 ARE, thereby circumventing the need for cell aggregation.In fact, TSA efficiently induced reporter gene expression in theabsence of both RA andaggregation.

To investigate the effect of TSA on endogenous gene expression, we performed Western blot analysis on TSA-treated cultures.Figure 1C shows that TSA efficiently induced the expression ofthe endogenous Hoxb1 gene, while PBX1 (Fig. 1C) and MEIS1 (datanot shown) showed a moderate increase over preexisting levels.Thus, TSA-treated cultures express all three homeoprotein familiesimplicated in activation through the Hoxb1 ARE. In contrast, TSAhad no effect on a stably integrated control transgene (p1230)that lacks the Hoxb1 ARE, establishing the specificity of thiseffect (Fig. 1B, inset). Together, these results suggest thatHOXB1-PBX complexes recruit HDACs in vivo to repress transcriptiondirected by the Hoxb1 ARE. TSA treatment inhibits HDAC activity,thereby inducing both the endogenous Hoxb1 gene and the b1-ARE-lacZreporter.

The Hoxb1 ARE used above is 150 bp long and may contain binding sites for TSA-responsive transcription factors other thanPBX or HOX proteins. To specifically test the response of HOX-PBXcomplexes to TSA, we transfected HEK293 cells with an artificialluciferase reporter, pML(5xHOX-PBX), driven solely by five HOX-PBXbinding sites in front of a minimal promoter. pML(5xHOX-PBX) wasrepressed fivefold relative to the parental vector pML lackingHOX-PBX binding sites (Fig. 2), again implicating HOX-PBX complexesin transcriptional repression. While pML was induced <2-fold byTSA, pML(5xHOX-PBX) was activated 12-fold (Fig. 2), further supportinga role for HDACs in repression mediated by HOX-PBX complexes.

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FIG. 2. PBX is required for the HOX-PBX response to TSA. pML(5xHOX-PBX), a reporter driven by five HOX-PBX binding sites, is repressed in transiently transfected HEK293 cells compared to pML, which lacks HOX-PBX binding sites. pML(5xHOX-PBX) is significantly activated by TSA (2 µM, 24 h) both in the absence or presence of overexpressed HOX and PBX1A proteins. Removal of residues 1 to 89 of PBX1A ( $Delta$ 1-89) greatly increases reporter activation by TSA. pML(5xHOX), containing five sites for monomeric HOX binding, is not repressed in 293 cells and is not further activated by TSA treatment. Overexpression of HOXA1 or HOXD4, but not of A1 WM-AA or D4 WM-AA, transactivates transcription in the presence of TSA. All transfections were repeated at least three times in duplicate except for the A1 WM-AA and D4 WM-AA experiments, which were done once in duplicate.

Overexpression of HOXB1, HOXA1, or HOXD4 enhanced the activation of pML(5xHOX-PBX) by TSA (Fig. 2), confirming the involvementof HOX proteins in this effect. In contrast, the TSA responsewas dampened by the overexpression of PBX1A (Fig. 2). Interestingly,deletion of the first 89 residues of PBX1A rendered the derivativeprotein highly TSA sensitive, resulting in an almost 100-foldactivation of pML(5xHOX-PBX). We suggest explanations for thiseffect inDiscussion.

PBX is required for repression by HOX-PBX and for the response to TSA. The above results implicate HOX proteins in transcriptional activation through HOX-PBX binding sites, whereas PBX had a repressiveeffect. To assess the importance of PBX for repression and theTSA response, we examined an independent reporter, pML(5xHOX),driven by monomeric HOX binding sites. In contrast to pML(5xHOX-PBX),pML(5xHOX) was not repressed in 293 cells and was not activatedby TSA (Fig. 2). This result argues that PBX is required for therepression observed on pML(5xHOX-PBX) and for activation by TSAon this reporter. Reciprocally, HOX proteins cannot activate transcriptionefficiently in the absence of a PBXpartner.

In a complementary test, we used derivatives of HOXA1 and HOXD4 harboring mutations in the conserved YPWM motif (A1 WM-AAand D4 WM-AA, respectively). This mutation has been previouslyshown not to affect the stability of HOXD4 (72) and to abolishinteraction between HOX and PBX proteins (66, 67, 76, 77).As shown in Fig. 2, while overexpression of HOXA1 or HOXD4 greatlyenhanced the TSA effect on pML(5xHOX-PBX), this was abolishedwith A1 WM-AA and D4 WM-AA. These findings demonstrate that interactionof HOX with PBX is required for the TSA response of pML(5xHOX-PBX).To explain these results, we propose a model whereby physicalinteraction between HOX and PBX is required for association withcoactivators and corepressors, respectively (seeDiscussion).

PBX1 interacts with class I HDACs. As shown above, PBX is required for TSA-sensitive repression mediated by HOX-PBX binding sites. The simplest explanation forthis finding is that PBX directly interacts with one or more HDACs.To test this, we performed immunoprecipitation experiments usingwhole-cell extracts from transfected 293 T cells. Flag-epitope-taggedHDAC1 and HDAC3, but not HDAC4, resulted in coprecipitation ofPBX1 (Fig. 3A). This interaction is specific and shows a preferencefor the class I HDACs by HOX-PBX complexes. More stringently,rabbit polyclonal antibodies that specifically recognize PBX1coprecipitated the endogenous HDAC1 and mSIN3B (Fig. 3B, lanes1 and 3). Interestingly, no interaction was observed with mSIN3A(Fig. 3B, lane 2) or with Mi2 $alpha$ or - $beta$ (data not shown). However,as shown in Fig. 3D (lane 2), N-CoR, known to repress transcriptionin an mSIN3A complex (58), coprecipitated with PBX1 in vivo.Thus, N-CoR/SMRT may associate with mSIN3B in the absence of mSIN3A.

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FIG. 3. The HOX-PBX complex associates with class I HDACs in vivo and represses transcription in a mSIN3B/N-CoR/SMRT-dependent manner. (A) PBX1 coprecipitates with class I HDACs (HDAC1 and HDAC3, lane 2 and 4) but not with HDAC4 (lane 3) or from cells transfected with the empty flag vector (F-control) (lane 1). Immunoprecipitations were done with lysates from 293 T cells cotransfected with plasmids expressing PBX1A and flag-tagged HDAC1 (F-HDAC1), F-HDAC3, F-HDAC4, or F-control. Flag-tagged proteins were immunoprecipitated with M2 beads (Sigma), and the precipitates were eluted with flag peptides (Sigma) and analyzed by Western blotting using rabbit polyclonal antibodies against PBX1 (Santa Cruz). "IP" and "WCE" denote immunoprecipitates and whole-cell extracts used in Western blot analysis. "W" denotes the antibody used in Western analysis. (B) Coprecipitation of endogenous HDAC1 and mSIN3B (but not mSIN3A) with rabbit polyclonal antibodies against PBX1. 293 T cells were transfected with a plasmid expressing PBX1A but not with plasmids expressing HDAC1, mSIN3B, or mSIN3A. Immunoprecipitates with anti-PBX1 antibodies (IP: $alpha$ -PBX1) were analyzed in Western blots with antibodies against HDAC1 (W: $alpha$ -HDAC1), mSIN3a (W: $alpha$ -mSIN3a), and mSIN3b (W: $alpha$ -mSIN3b). (C) The repression of pML(5xHOX-PBX) in 293 T cells is exerted by N-CoR/SMRT-corepressor complexes. Overexpression of either N-CoR or SMRT further repressed pML(5xHOX-PBX). This repression can be partially relieved by sequestering the endogenous N-CoR/SMRT with overexpressed estrogen receptor (ER) bound to the estrogen antagonist TOT (see Materials and Methods). (D) Immunoprecipitation of PBX1 from cells expressing flag-tagged N-CoR (F-N-CoR, lane 2) but not from cells transfected with the empty flag vector (F-control, lane 1).

To functionally characterize these interactions, we examined the effects of N-CoR and SMRT on pML(5xHOX-PBX). As shown inFig. 3C, overexpression of either N-CoR or SMRT potentiated therepression observed with pML(5xHOX-PBX) in 293 T cells. Overexpressionof an antagonist-bound estrogen receptor, in an attempt to titratethe endogenous levels of N-CoR/SMRT (41), resulted in a partialrelief of repression of pML(5xHOX-PBX). These data suggest thatN-CoR/SMRT complexes are recruited by HOX-PBX within the cellto exert significant repression effects on downstreamtargets.

Region from residues 89 to 172 in the PBX1 N terminus interacts with HDAC1. In PBX1, three N-terminal repression domains (corresponding to regions B, C, and D in Fig. 4A) have been previously mapped(45). To directly characterize whether one of these repressiondomains recruits the HDAC complex, we generated multiple in-framedeletions in PBX1A (Fig. 4A) and examined the in vivo associationwith HDAC1. Immunoprecipitation studies were carried out withextracts from 293 T cells cotransfected with plasmids expressingflag-tagged HDAC1 along with PBX1A deletion derivatives. Followingimmunoprecipitation with anti-flag antibodies, the precipitateswere analyzed by Western analysis using polyclonal antibodiesagainst PBX1 or anti-HA antibodies in the cases of $Delta$ 89-HA and89-172-HA. Fig. 4B shows that the PBX1 N terminus ( $Delta$ C232) is sufficientfor HDAC1 binding.

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FIG. 4. Region C of PBX1A is responsible for the interaction with HDAC1. (A) Schematic representations of wild-type PBX1A and PBX1A deletion mutants. The subdivision of the PBX1A N terminus into four domains labeled A, B, C, and D is as previously described (45). The striped rectangle indicates the position of the HA tag in $Delta$ 1-89 and in HA-89-172. (B) The PBX1A N terminus interacts with HDAC1. Binding studies similar to those described in the legend to Fig. 3A were carried out for PBX1A and PBX1A mutants with flag-tagged HDAC1 immunoprecipitated on M2 beads and eluted with flag peptide. Anti-PBX1 antibodies were used for the Western analysis. (C) Regions A and B of PBX1A are dispensable for interaction with HDAC1 and -3. The experiment was done as described in the legend to panel B except that the $Delta$ 1-89 mutant was tagged with the HA epitope and was recognized in Western analysis by anti-HA antibodies (Babco). The black arrowhead indicates HDAC1, the white arrowhead indicates HDAC3, and the asterisk indicates an HDAC1 degradation product. (D) HDAC1 coprecipitates with the region from residues 89 to 172 of PBX1A. Cells were transfected with a vector expressing flag-tagged HDAC1 and either an empty HA vector (HA-control) or one expressing the HA-tagged region from residues 89 to 172 of PBX1. Immunoprecipitation (IP) experiments were carried out with anti-HA antibodies, and anti-flag antibodies were used in the Western analysis.

$Delta$ 89 is highly responsive to TSA (Fig. 2), suggesting that the HDAC interaction region in PBX1A is C terminal to residue 89.As shown in Fig. 4C, $Delta$ 89-HA associated with HDAC1 and HDAC3 inwhole-cell extracts, mapping the region of interaction with HDAC1to PBX1A region C or D. Two deletions in region D were thereforetested and found to be dispensable for HDAC1 binding ( $Delta$ 137-160and $Delta$ 160-232, Fig. 4A and B). These data imply that region C isimportant for the recruitment of the HDAC complex byPBX1.

A deletion mutant of region C was not stable in mammalian cells. To address whether region C is sufficient for interactionwith HDAC1, we used anti-HA antibodies to immunoprecipitate afusion protein containing the HA epitope fused in frame to residues89 to 172 spanning region C of PBX1A. As seen in Fig. 4D, HDAC1coprecipitated with HA-89-172 (lane 2) but not with an HA control(lane 1). The above data indicate that, while the region B repressionmechanism is TSA insensitive, region C recruits HDACs to represstranscription.

The HOXD4 activation domain binds the HAT-C/H3 domain of CBP. Treatment with TSA led to large increases in transcription from natural and artificial enhancers bearing HOX-PBX binding sites(Fig. 1 and 2). Activation of pML(5xHOX-PBX) exceeded a simpleloss of repression relative to pML (Fig. 2A). These results showthat TSA reveals a transcriptional activation function of theHOX-PBX heterodimer. Transcriptional activation is achieved throughrecruitment of coactivators by enhancer-bound proteins. One suchcoactivator is CBP. To assess its involvement in transcriptionalactivation by HOX-PBX complexes, we overexpressed CBP in 293 Tcells. CBP stimulated expression from pML(5xHOX-PBX) 10- to 12-fold,similar to the activation obtained by TSA treatment (Fig. 5A,lane 2). This result suggested that PBX, HOX, or both recruitedCBP to target promoters.

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FIG. 5. CBP enhances the transactivation potential of HOX-PBX complexes and is required to transduce PKA signaling. (A) pML(5xHOX-PBX) is activated by overexpression of CBP in 293 T cells and is superactivated by the catalytic domain of PKA. Activation by PKA is inhibited by overexpression of E1A. (B) A fusion of the N terminus of HOXD4 to the GAL4 DNA-binding domain (GAL4-HOXD4N) is able to transactivate transcription from a heterologous promoter driven by 5xGAL4 binding sites [pML(5xUAS)] (lanes 1 and 2, black bars). CBP potentiates the transactivation function of HOXD4N on this reporter (lane 3, black bar) in a manner sensitive to E1A (white bar) but not to E1A $Delta$ N (dotted bar), a mutant deficient in CBP binding. PKA stimulates HOXD4N transactivation in a CBP-dependent manner (lanes 4 and 5).

We have previously characterized an activation domain in the proline-rich N-terminal half of HOXD4 (73). We therefore testedwhether the HOXD4 activation domain (HOXD4N, residues 3 to 141)could recruit CBP to a target promoter. Figure 5B (lanes 1, 2,and 3, black bars) shows that overexpression of CBP potentiatestransactivation by a GAL4-HOXD4N fusion protein on the GAL4-responsivereporter pML(5xUAS). In contrast, depletion of endogenous CBPby overexpression of the oncoprotein E1A neutralizes the coactivationeffect seen with overexpressed CBP. E1A also inhibits the initialactivation observed with HOXD4N (Fig. 5B, compare white bars inlanes 2 and 3 to black bars in lanes 1, 2, and 3). A deletionmutant of E1A that cannot bind CBP is unable to affect transcriptionsignificantly (dotted bars in Fig. 5B). These results show thatthe transactivation function of HOXD4N is mediated by endogenousCBP. We also note that E1A interacts with the coactivator p300through this same domain. None of our data excludes an interactionbetween HOX proteins and p300, in addition to CBP. Likewise, PCAFis expected to bind CBP in association with HOX (89).

In vivo mapping studies were carried out to determine the respective domains of interactions between HOXD4 and CBP. A fusionof GAL4 to the HOXD4 N terminus (GAL4-HOXD4N) but not to the Cterminus (GAL4-HOXD4C) coprecipitated with CBP, consistent withthe N-terminal transactivation function of HOXD4 (Fig. 6A, lanes1 and 2). To map the domains in CBP required for HOX binding,immunoprecipitation experiments were carried out with extractsfrom 293 T cells cotransfected with plasmids expressing GAL4-HOXD4Nand one of four HA-tagged CBP domains: CBP-N, CBP-KIX, CBP-HAT-C/H3,or CBP-C (Fig. 6B). Analysis of the precipitates was carried outby Western blot analysis with anti-HA antibodies. The four CBPdomains used in this experiment were expressed at equivalent amountsin 293 T cells (data not shown). Figure 6B shows that the HAT-C/H3domains of CBP constitute the region of interaction with HOXD4N.

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FIG. 6. (A) Interactions between the HOXD4 N terminus and CBP. GAL4-HOXD4N or GAL4-HOXD4C were immunoprecipitated with antibodies against the GAL4 DBD. Interaction with HA-tagged CBP (HA-CBP) in the presence or in the absence of overexpressed PKA was assessed by Western analysis using anti-HA antibodies. (B) The HOXD4 N terminus coprecipitates with the CBP HAT-C/H3 domains. Immunoprecipitation studies were performed on whole-cell extracts from 293 T cells cotransfected with GAL4-HOXD4N along with four HA-tagged domains of CBP: HA-CBP-N (amino acids 1 to 460), HA-CBP-KIX (amino acids 460 to 662), HA-CBP-HAT-C/H3 (amino acids 1450 to 1903), or HA-CBP-C (amino acids 2040 to 2170). Immunoprecipitation (IP) was performed with antibodies against the GAL4 DBD, and the CBP domains were detected by Western analysis using anti-HA antibodies. The schematic representation of the CBP protein is as described by Chariot et al. (14).

PKA signaling stimulates HOX-PBX promoters. The above results show that PBX and HOX proteins directly contact transcriptional corepressors and coactivators, respectively.What determines whether the HOX-PBX complex will have a net activatingor repressive effect on gene expression? Our studies in P19 ECcells show that aggregation provides a signal that converts HOX-PBXcomplexes from repressors to activators. This conversion is dependenton cell aggregation. Among other possibilities, aggregation mayincrease the concentration of secreted growth factors or allowpresentation of surface-bound ligands to receptors on adjacentcells. Signaling via cyclic AMP (cAMP) second messenger is mediatedby PKA. PKA has been implicated in the activation function ofa number of transcription factors, including the homeoproteinPIT1. Given the known role of CBP in mediating the effects ofPKA on transcriptional activation (2, 24), we tested theability of PKA to convert HOX-PBX complexes from transcriptionalrepressors toactivators.

Overexpression of the catalytic domain of PKA significantly stimulated pML(5xHOX-PBX) in 293 T cells (Fig. 5A). This effectwas mediated through HOX-PBX binding sites since PKA had a minimaleffect (2.6-fold) on pML lacking the HOX-PBX binding sites. Thisresult suggests a link between the activation of the intracellularcAMP signal transduction pathway and the activity of HOX-PBXcomplexes.

We examined the impact of PKA signaling on transactivation of the GAL4-responsive reporter pML(5xUAS) by the GAL4-HOXD4N fusionprotein. Figure 5B (lane 4) shows that PKA stimulated this reporter500-fold in a HOXD4N-dependent manner. The PKA stimulation requiresCBP since depletion of endogenous CBP by overexpression of E1Ainhibited this effect (lanes 4 and 5, white bars). Overexpressionof PKA along with GAL4-HOXD4N and CBP-HA resulted in increasedamounts of CBP coprecipitates with equivalent amounts of HOXD4N(Fig. 6A, lane 3). These data suggest that the recruitment ofCBP by the activation domain of HOXD4 is facilitated in the presenceof PKA. This further suggests a mechanism by which DNA-bound HOX-PBXcomplexes could be switched from repressors to activators throughenhanced association withCBP.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Two observations suggested to us that HOX-PBX complexes may recruit transcriptional corepressors to target promoters. First,the Hoxb1 ARE is inactive in RA-treated P19 cell monolayers despitethe presence of HOXB1 and PBX1 but is activated in response tothe HDAC inhibitor TSA (Fig. 1). Second, repression by multimerizedHOX-PBX binding sites is likewise alleviated by TSA treatment(Fig. 2). Transcriptional activation through the Hoxb1 ARE ormultimerized HOX-PBX binding sites further suggested that HOX-PBXcomplexes recruit transcriptional coactivators. In support ofthis suggestion, a repression domain in the PBX1 N terminus bindsa corepressor complex containing class I HDACs in associationwith N-CoR/SMRT and mSIN3B (Fig. 3 and 4). Conversely, the proline-richactivation domain of HOXD4 binds the CBP coactivator. We providedadditional evidence that the HOX-PBX complex can be switched froma repressor to an activator of transcription through the actionof signaling cascades (Fig. 5, 6, and 7). Specifically, the HOX-PBXcomplex becomes a CBP-dependent transcriptional activator in responseto PKA. Thus, the transcriptional activity of the HOX complexin a specific tissue at a given developmental stage may come underthe control of signaling cues such as intracellularcAMP.

Repression of HOX-PBX targets is mediated by PBX-corepressor interactions. PBX1 has been previously shown to possess three repression domains in its N terminus (45). Our results indicate that PBX1represses transcription through both TSA-sensitive and -insensitivemechanisms. We found that the first N-terminal repression domainof PBX1 (domain B) represses transcription in a TSA-resistantfashion. By contrast, the second N-terminal repression domain(within region C) associates with class I HDACs. Recently, othershave shown that PBX1A binds N-CoR and SMRT through its C terminus(4). The set of PBX1A derivatives employed here does not refutethis finding. Rather, the cumulative data suggest that PBX1A containsmore than one docking site for corepressorcomplexes.

The corepressors N-CoR and SMRT are known to repress transcription in an mSIN3A complex (58). In addition, SMRT has beenshown to function in an HDAC3 complex (28). The presence ofmSIN3B and not mSIN3A in the corepressor complex recruited byPBX1 is a novel indication of an interaction between N-CoR/SMRTandmSIN3B.

Overexpression of wild-type PBX1A inhibits TSA-mediated activation of a reporter bearing multiple HOX-PBX binding sites (Fig.2, lane 5). By contrast, removal of the first 89 residues of PBX1A,or overexpression of HOX proteins, confers a strong TSA response.Two nonexclusive explanations are possible. First, residues 1to 89 of PBX1A may harbor a TSA-insensitive repression domain.This could be mediated by direct contact to a repressor, or indirectlythough members of the MEIS/PREP family which bind PBX proteinsthrough this N-terminal domain (11). This could explain theenhanced TSA response with $Delta$ 1-89 but would not explain the dampenedresponse with wild-type PBX1A. Another explanation is that increasedlevels of PBX1A promote the formation of PBX-PBX homodimers atthe target promoter. Such homodimers have been described in theliterature (8, 59) and would be expected to form on the multimerizedbinding sites in pML(5xHOX-PBX). In theory, the PBX homodimerwould compete with HOX-PBX heterodimers for DNA binding, recruitingonly corepressors to the target promoter and thereby dampeningthe response to TSA. Deletion of the first 89 residues from PBX1Aseverely impairs homodimerization (K. Shanmugam and M. S. Featherstone,unpublished observations) without affecting heterodimerizationwith at least some HOX partners (77). Thus, $Delta$ 1-89 would promotebinding by HOX-PBX heterodimers at the expense of PBX homodimers,resulting in more efficient recruitment ofcoactivators.

Residues 1 to 89 of PBX1 are deleted in the oncoprotein E2A-PBX (32). Thus, the increased transcriptional activation functionand the concomitant oncogenicity of E2A-PBX may be due to boththe loss of a repression domain, as well as to the recruitmentof HATs by the E2A activation domain (16, 33, 52). The HDAC1binding domain in PBX1 (domain C) is retained in E2A-PBX. Consistentwith this, TSA potentiates the activation observed with E2A-PBX(unpublished observations). Thus, treatment with TSA may potentiateB-celltransformation.

Domain C of PBX1 spans a short stretch of nine alanine residues and impinges on the conserved PBC-A and -B domains. The PBCdomains are highly conserved across species. In contrast, thealanine stretch is conserved in mammals and flies but is absentin the C. elegans CEH-20 protein. Monotonic alanine regions havebeen implicated in repressor function (29, 44, 47); however,at this time the highly conserved portions of PBC-A and -B areequally plausible candidates for direct interaction with repressorcomplexes.

CBP modifies HOXD4 function and transduces PKA stimulation of HOX-PBX promoters. We have shown that the proline-rich activation domain of HOXD4 physically interacts with the HAT-C/H3 domain of the CBP coactivator.Interestingly, the interaction between HOXD4 and CBP seems tobe conserved through evolution, since Deformed, the Drosophilaorthologue of Hoxd4, has been shown genetically to interact withNejire, encoding a transcriptional adapter belonging to the CBP/p300family (22). A previous study has shown physical interactionbetween CBP and the N terminus of HOXB7 (14). Using truncatedversions of each protein in vitro and in transfections, theirsites of interaction were mapped to the HOXB7 N terminus and tworegions in CBP, including the C/H3 domain and the extreme C terminus.Together with another study showing interaction between the Nterminus of the HOX-like protein PDX and the CBP C/H3 domain (4),these findings suggest a common mechanism used by homeoproteinsto activatetranscription.

To date, four Hox genes, namely Hoxb1, Hoxa4, Hoxb4, and Hoxd4, have been shown to contain RAREs and AREs in their flankingregions (26, 30, 39, 51, 56, 63, 69, 70, 83,92). The HOX interaction region in CBP centering on the C/H3domain is different from the nuclear receptor interaction region(RID) (10, 31). This suggests that one CBP molecule couldsimultaneously bind both retinoid receptor and HOX family members.This may result in synergistic recruitment of CBP to Hox genepromoters, thereby integrating the activities of retinoid receptorsand HOXproteins.

Interactions between HOX and CBP can explain some of the phenotypes resulting from Cbp loss-of-function mutations. In humans,the Rubinstein-Taybi syndrome is caused by point mutations inthe Cbp gene and is characterized by craniofacial deformations,broad thumbs, broad big toes, severe mental retardation, and increasedtumor incidence (65). In the mouse, targeted disruptions ofCbp and p300 have revealed the importance of these cofactors inembryonic development (90). In Drosophila, mutations in Cbpcause embryonic lethality as well as pattern defects (1). Someof these defects are reminiscent of those caused by mutationsin Hox genes (38) and can be partly explained by the findingthat CBP modifies HOX transcriptionalactivities.

Genetic and molecular studies in Drosophila have led to a model whereby the N-terminal activation domain of HOX proteins ismasked due to direct or indirect contact with the HOX homeodomain(42, 43). The model further suggests that this inhibitionis relieved upon a conformational change provoked by cooperativeDNA binding of HOX with PBX. In this model, DNA-bound HOX monomersare repressors, while HOX-EXD (or HOX-PBX) heterodimers are activators.Our data are consistent with aspects of this model. First, TSAis able to activate a promoter driven by HOX-PBX dimer bindingsites but not one driven by HOX monomer binding sites. Second,mutations in the HOX YPWM motif that abrogate interaction withPBX also abolish the TSA response, even on HOX-PBX cooperativebinding sites. Both of these observations would be expected ifPBX is required to unmask the HOX activation domain, thereby permittinginteraction with CBP. However, the very fact that the HOX-PBXcomplex is responsive to TSA suggests a repressor function mediatedby interaction with HDACs, consistent with data reported hereand elsewhere that PBX functions as a repressor and binds corepressors(4, 45).

In addition, we did not observe transcriptional repression by HOX monomers under our conditions. HOX monomer binding sitesdo not repress basal transcription [Fig. 2, compare pML to pML(5xHOX)],and HOX mutants that are incapable of interacting with PBX partnersdo not behave as transcriptional repressors (Fig. 2) (72). Rather,our data suggest that the HOX-PBX complex can act as both a transcriptionalrepressor and activator, depending on the cellular context (Fig.7). We argue that this context can be influenced by cell-cellsignaling, since aggregation is required to activate the Hoxb1ARE in RA-treated P19 cells. Monolayers of P19 cells can be induceddown the neural pathway by combined treatment with forskolin,an activator of PKA signaling, and a factor secreted by cellsresembling primitive streak mesoderm (71). This is consistentwith a role for PKA in the activation of the Hoxb1 ARE. We alsonote that aggregation of P19 cells has been proposed to influencethe activity of the MYOD muscle-specific transcription factorthrough effects on chromatin (3).

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FIG. 7. A model for activation and repression by HOX-PBX complexes. The N-terminal activation and repression domains of HOX and PBX proteins are believed to make intramolecular contact with their respective homeodomains (8, 42, 43, 59, 74). Heterodimerization on cooperative sites on DNA, and perhaps additional interactions with members of the MEIS/PREP family, exposes HOX and PBX N termini, thereby freeing them for interaction with coactivators and corepressors such as CBP and HDAC1 and -3. Under some cellular contexts, the net activity of bound corepressors exceeds that of the activators (bottom, "net repressor function"). However, in response to enhanced PKA signaling or P19 cell aggregation, increased coactivator and/or decreased corepressor function shifts the balance toward net activation (top). This could be accomplished by an increase in the amount of coactivator or by increased affinity for the HOX N terminus. In parallel, decreases in the amount or affinity of corepressor for PBX could contribute to the switch. Treatment with TSA would exert the same overall effect by inhibiting bound HDACs. The model is simplified and does not exclude other possible interactions. The black vertical arrows denote increases or decreases in HAT or HDAC activity. AD, HOX activation domain; RD, PBX repression domain C; black box, homeodomain; small white circle, HOX YPWM motif.

Our finding that CBP-HOX activation of downstream targets is significantly enhanced by PKA suggests a mechanism for conversionof HOX-PBX complexes from transcriptional repressors to activators.PKA was previously shown to be important for the transactivationof bovine CYP17 by PBX, as well as the oncoprotein E2A-PBX, viaa cAMP response sequence (CRS) (61). The CRS in the promoterof CYP17 is very closely linked to a PBX response sequence thatshould accommodate cooperative binding by HOX-PBX in vitro. Thissuggests that the CRS response to PKA could be mediated by a HOXpartner viaCBP.

CBP contains a defined PKA phosphorylation site at serine 1772 shown to be important for mediating PKA-stimulated activationby the homeoprotein PIT1 (85). Our results likewise suggestthat CBP phosphorylation by PKA is the signal transduction steprequired for HOXD4 to activate transcription in response to increasedintracellular cAMP. We demonstrated increased association of theHOXD4 activation domain with CBP upon increased PKA signaling(Fig. 5A). How is this achieved? The levels of CBP are greatlyincreased in 293 cells expressing the catalytic subunit of PKA(unpublished observations). This increase may be sufficient toaccount for the greater association between HOXD4 and CBP uponPKAstimulation.

A role for PKA in HOX function in the embryo has not been clearly demonstrated. However, patterning by the hedgehog signalingpathway in flies and mice involves antagonizing the PKA pathway(19, 60). Our results suggest that PKA may also impinge onpatterning mediated by the HOX family. Hox genes are known todetermine the morphogenetic outcome of cell signaling in fly imaginaldiscs (64). In C. elegans, genetic studies have shown that aHOX protein determines the developmental consequences of RAS signaling(48). On theoretical grounds, HOX proteins were predicted tointerpret cell signaling events in vertebrates as well (17).Our results support thissuggestion.

In summary, we have demonstrated that HOX-PBX can function as an activator or a repressor through differential interactionswith coregulators. Moreover, we have shown that PKA serves asa signaling switch that converts HOX-PBX from repressor to activator,implying that cell signaling is an important determinant of HOX-PBXfunction in the patterning of the animalembryo.

	ACKNOWLEDGMENTS

We thank C. Largman for a gift of anti-HOXB1 antibody and R. Krumlauf for the p1230 lacZ reporter. We are grateful to A. Laiand P. Branton for their advice and gifts of vectors for F-HDAC1,F-HDAC3, E1A, and E1A $Delta$ N. We thank A. Tremblay and V. Giguèrefor gifts of vectors for N-CoR, SMRT, ER, and the CBP domains;Y. Zhang for the Mi2 antibodies; and members of the Featherstonelab for helpfuldiscussions.

M.S. is the recipient of a Medical Research Council of Canada Studentship. X.-J.Y. is a scholar of the Medical Research Councilof Canada. M.S.F. is a Chercheur-Boursier of the Fonds de la Rechercheen Santé du Québec. This work was funded by grants to X.-J.Y.and M.S.F. from the Medical Research Council ofCanada.

	FOOTNOTES

^* Corresponding author. Mailing address: McGill Cancer Centre, McGill University, McIntyre Medical Sciences Bldg., Rm. 714,3655 Promenade Sir William Osler, Montreal, Quebec, Canada H3G1Y6. Phone: (514) 398-8937. Fax: (514) 398-6769. E-mail: mfeather{at}med.mcgill.ca.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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44. Licht, J. D., W. Hanna-Rose, J. C. Reddy, M. A. English, M. Ro, M. Grossel, R. Shaknovich, and U. Hansen. 1994. Mapping and mutagenesis of the amino-terminal transcriptional repression domain of the Drosophila Kruppel protein. Mol. Cell. Biol. 14:4057-4066[Abstract/Free Full Text].

45. Lu, Q., and M. P. Kamps. 1996. Selective repression of transcriptional activators by Pbx1 does not require the homeodomain. Proc. Natl. Acad. Sci. USA 93:470-474[Abstract/Free Full Text].

46. Lufkin, T., A. Dierich, M. LeMeur, M. Mark, and P. Chambon. 1991. Disruption of the Hox-1.6 homeobox gene results in defects in a region corresponding to its rostral domain of expression. Cell 66:1105-1119[CrossRef][Medline].

47. Mailly, F., G. Berube, R. Harada, P. L. Mao, S. Phillips, and A. Nepveu. 1996. The human cut homeodomain protein can repress gene expression by two distinct mechanisms: active repression and competition for binding site occupancy. Mol. Cell. Biol. 16:5346-5357[Abstract].

48. Maloof, J. N., and C. Kenyon. 1998. The Hox gene lin-39 is required during C. elegans vulval induction to select the outcome of Ras signaling. Development 125:181-190[Abstract].

49. Mann, R. S., and M. Affolter. 1998. Hox proteins meet more partners. Curr. Opin. Genet. Dev. 8:423-429[CrossRef][Medline].

50. Mann, R. S., and S.-K. Chan. 1996. Extra specificity from extradenticle: the partnership between HOX and PBX/EXD homeodomain proteins. Trends Genet. 12:258-262[CrossRef][Medline].

51. Marshall, H., M. Studer, H. Pöpperl, S. Aparicio, A. Kuriowa, S. Brenner, and R. Krumlauf. 1994. A conserved retinoic acid response element required for early expression of the homeobox gene Hoxb-1. Nature 370:567-571[CrossRef][Medline].

52. Massari, M., P. Grant, M. G. Pray-Grant, S. L. Berger, J. L. Workman, and C. Murre. 1999. A conserved motif present in a class of helix-loop-helix proteins activates transcription by direct recruitment of the SAGA complex. Mol. Cell 4:63-73[CrossRef][Medline].

53. McBurney, M. W., X. Yang, K. Jardine, and M. Cormier. 1998. A role for RNA processing in regulating expression from transfected genes. Somat. Cell Mol. Genet. 24:203-215[CrossRef][Medline].

54. McGinnis, W., and R. Krumlauf. 1992. Homeobox genes and axial patterning. Cell 68:283-302[CrossRef][Medline].

55. Monica, K., N. Galili, J. Nourse, D. Saltman, and M. L. Cleary. 1993. PBX2 and PBX3, new homeobox genes with extensive homology to the human proto-oncogene PBX1. Mol. Cell. Biol. 11:6149-6157.

56. Morrison, A., M. C. Moroni, L. Ariza-McNaughton, R. Krumlauf, and F. Mavilio. 1996. In vitro and transgenic analysis of a human hoxd4 retinoid-responsive enhancer. Development 122:1895-1907[Abstract].

57. Moskow, J. J., F. Bullrich, K. Huebner, I. O. Daar, and A. M. Buchberg. 1995. Meis1, a PBX1-related homeobox gene involved in myeloid leukemia in BXH-2 mice. Mol. Cell. Biol. 15:5434-5443[Abstract].

58. Nagy, L., H. Y. Kao, D. Chakravarti, R. J. Lin, C. A. Hassig, D. E. Ayer, S. L. Schreiber, and R. M. Evans. 1997. Nuclear receptor repression mediated by a complex containing SMRT, mSin3A, and histone deacetylase. Cell 89:373-380[CrossRef][Medline].

59. Neuteboom, S. T. C., and C. Murre. 1997. Pbx raises the DNA binding specificity but not the selectivity of Antennapedia Hox proteins. Mol. Cell. Biol. 17:4696-4706[Abstract].

60. Noveen, A., T. X. Jiang, and C. M. Chuong. 1996. cAMP, an activator of protein kinase A, suppresses the expression of sonic hedgehog. Biochem. Biophys. Res. Commun. 219:180-185[CrossRef][Medline].

61. Ogo, A., M. R. Waterman, M. P. Kamps, and N. Kagawa. 1995. Protein kinase A-dependent transactivation by the e2a-pbx1 fusion protein. J. Biol. Chem. 270:25340-25343[Abstract/Free Full Text].

62. Oulad-Abdelghani, M., C. Chazaud, P. Bouillet, V. Sapin, P. Chambon, and P. Dollé. 1997. Meis2, a novel mouse Pbx-related homeobox gene induced by retinoic acid during differentiation of P19 embryonal carcinoma cells. Dev. Dynam. 210:173-183[CrossRef][Medline].

63. Packer, A. I., D. A. Crotty, V. A. Elwell, and D. J. Wolgemuth. 1998. Expression of the murine Hoxa4 gene requires both autoregulation and a conserved retinoic acid response element. Development 125:1991-1998[Abstract].

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44.	Licht, J. D., W. Hanna-Rose, J. C. Reddy, M. A. English, M. Ro, M. Grossel, R. Shaknovich, and U. Hansen. 1994. Mapping and mutagenesis of the amino-terminal transcriptional repression domain of the Drosophila Kruppel protein. Mol. Cell. Biol. 14:4057-4066[Abstract/Free Full Text].
45.	Lu, Q., and M. P. Kamps. 1996. Selective repression of transcriptional activators by Pbx1 does not require the homeodomain. Proc. Natl. Acad. Sci. USA 93:470-474[Abstract/Free Full Text].
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47.	Mailly, F., G. Berube, R. Harada, P. L. Mao, S. Phillips, and A. Nepveu. 1996. The human cut homeodomain protein can repress gene expression by two distinct mechanisms: active repression and competition for binding site occupancy. Mol. Cell. Biol. 16:5346-5357[Abstract].
48.	Maloof, J. N., and C. Kenyon. 1998. The Hox gene lin-39 is required during C. elegans vulval induction to select the outcome of Ras signaling. Development 125:181-190[Abstract].
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51.	Marshall, H., M. Studer, H. Pöpperl, S. Aparicio, A. Kuriowa, S. Brenner, and R. Krumlauf. 1994. A conserved retinoic acid response element required for early expression of the homeobox gene Hoxb-1. Nature 370:567-571[CrossRef][Medline].
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53.	McBurney, M. W., X. Yang, K. Jardine, and M. Cormier. 1998. A role for RNA processing in regulating expression from transfected genes. Somat. Cell Mol. Genet. 24:203-215[CrossRef][Medline].
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