The HAND1 Basic Helix-Loop-Helix Transcription Factor Regulates Trophoblast Differentiation via Multiple Mechanisms

doi:10.1128/MCB.20.2.530-541.2000

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Molecular and Cellular Biology, January 2000, p. 530-541, Vol. 20, No. 2
0270-7306/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The HAND1 Basic Helix-Loop-Helix Transcription Factor Regulates Trophoblast Differentiation via Multiple Mechanisms

Ian C. Scott,¹^,² Lynn Anson-Cartwright,¹ Paul Riley,¹ Danny Reda,¹ and James C. Cross¹^,²^,³^,^*

Program in Development and Fetal Health, Samuel Lunenfeld Research Institute, Mount Sinai Hospital,¹ and Departments of Molecular and Medical Genetics² and Obstetrics and Gynaecology,³ University of Toronto, Toronto, Ontario Canada

Received 4 May 1999/Returned for modification 25 June 1999/Accepted 11 October 1999

	ABSTRACT

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The basic helix-loop-helix (bHLH) transcription factor genes Hand1 and Mash2 are essential for placental development in mice.Hand1 promotes differentiation of trophoblast giant cells, whereasMash2 is required for the maintenance of giant cell precursors,and its overexpression prevents giant cell differentiation. Wefound that Hand1 expression and Mash2 expression overlap in theectoplacental cone and spongiotrophoblast, layers of the placentathat contain the giant cell precursors, indicating that the antagonisticactivities of Hand1 and Mash2 must be coordinated. MASH2 and HAND1both heterodimerize with E factors, bHLH proteins that are theDNA-binding partners for most class B bHLH factors and which arealso expressed in the ectoplacental cone and spongiotrophoblast.In vitro, HAND1 could antagonize MASH2 function by competing forE-factor binding. However, the Hand1 mutant phenotype cannot besolely explained by ectopic activity of MASH2, as the Hand1 mutantphenotype was not altered by further mutation of Mash2. Interestingly,expression of E-factor genes (ITF2 and ALF1) was down-regulatedin the trophoblast lineage prior to giant cell differentiation.Therefore, suppression of MASH2 function, required to allow giantcell differentiation, may occur in vivo by loss of its E-factorpartner due to loss of its expression and/or competition fromHAND1. In giant cells, where E-factor expression was not detected,HAND1 presumably associates with a different bHLH partner. Thismay account for the distinct functions of HAND1 in giant cellsand their precursors. We conclude that development of the trophoblastlineage is regulated by the interacting functions of HAND1, MASH2,and theircofactors.

	INTRODUCTION

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The placenta is critical for the intrauterine survival of mammalian embryos. In mice, mutations that severely disrupt placentationor establishment of the chorioallantoic circulation result inembryonic lethality by day 10.5 of gestation (E10.5). Defectsin placentation also contribute to diseases of human pregnancy,including spontaneous abortion and preeclampsia (11). However,surprisingly little is known regarding the molecular events thatregulate development of the trophoblast cell lineage, the epithelialcomponent of the placenta. At the blastocyst stage, trophoblastcells in contact with the inner cell mass (polar trophectoderm)continue to proliferate and later contribute to the chorion andectoplacental cone (24). In contrast, trophoblast cells distalto the inner cell mass (mural trophectoderm) terminally differentiateto form primary trophoblast giant cells. While mitotically arrested,these cells undergo continued rounds of DNA synthesis (endocycles),thereby acquiring their characteristic giant polyploid nuclei(54). Secondary giant cells subsequently arise due to differentiationof precursor cells present in the ectoplacental cone and, laterin gestation, the spongiotrophoblast (17). Trophoblast giantcells participate in a number of processes critical to a successfulpregnancy, including blastocyst implantation, remodeling of thematernal decidua, and secretion of hormones that regulate bothfetal and maternal development (13).

A limited number of genes have been shown to play direct roles in early trophoblast development (for reviews, see references39 and 46). Hand1 and Mash2 encode members of the basic helix-loop-helix(bHLH) transcription factor family, which regulate the determinationand differentiation of several cell lineages (1). Mash2 mutantmouse conceptuses arrest at E10.5 due to placental defects thatinclude an absence of the spongiotrophoblast layer (derived fromtrophoblast of the ectoplacental cone), excess trophoblast giantcells, and a poorly developed labyrinthine layer (18, 50).Mash2 function is thus required to maintain spongiotrophoblastat the expense of giant cell differentiation. In contrast, Hand1mutants arrest at E7.5 due primarily to placental defects thatinclude a block in trophoblast giant cell differentiation anda smaller ectoplacental cone (38). These factors also have oppositeactivities when overexpressed in the Rcho-1 trophoblast cell line.While Hand1 expression promotes giant cell differentiation, Mash2inhibits this process (12, 25). As Hand1 and Mash2 have apparentlyopposing roles in trophoblast development, we wished to determinehow their activities are coordinatelyregulated.

Different mechanisms could in theory ensure that only Hand1 or Mash2 is active in a given cell. One possibility is that thetwo factors are expressed in nonoverlapping trophoblast subpopulations.Consistent with this model, Mash2 expression is broadened in Hand1mutants to encompass cells normally fated to differentiate intosecondary trophoblast giant cells (38), indicating that Hand1is essential for repressing Mash2 expression at the onset of giantcell differentiation. While transcripts of Hand1 (12, 15,19) and Mash2 (18, 32, 41) have been previously localizedin the placenta, these separate studies did not resolve if theyare coexpressed in individual trophoblast subtypes. Alternatively,HAND1 and MASH2 may be coexpressed, but they could compete foran essential cofactor. Members of the bHLH family dimerize viatheir HLH domains, allowing the two basic domains to bind DNA(52). Both HAND1 and MASH2 form heterodimers with E factors,the obligate partners of most bHLH factors (12, 23). It istherefore possible that HAND1 and MASH2, if present in the samecell, compete for the same E-factor partners, with the relativeabundance and dimerization affinities of HAND1 and MASH2 determiningwhich factor is functional. The different complexes could alsocompete for DNA-binding sites. MASH2-E-factor dimers bind to andactivate transcription from E-box sequences (CANNTG) (23). HAND1-E-factorcomplexes bind to a different consensus sequence (NNTCTG) (19),which has some overlap with E-box sequences. Thus, it is possiblethat HAND1 and MASH2 complexes bind to common sequences. If theydo, competition for shared sites would ensure that only one ofthese factors is active at a given time. In this study, we examinedeach of these possible mechanisms. The results demonstrate thatHand1 and Mash2 are coexpressed in the ectoplacental cone andspongiotrophoblast, intermediate trophoblast subpopulations. Invitro, HAND1 can inhibit MASH2 activity by virtue of competitionfor E-factor partners. However, analysis of Hand1/Mash2 compoundmutants indicates that Hand1 has a distinct role independent ofits effects on Mash2. Regulated expression of E-factor genes wasalso observed, a feature that may further compartmentalize Hand1and Mash2 functions during trophoblastdevelopment.

	MATERIALS AND METHODS

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Plasmids. pBS-ALF1B was constructed by ligating a 670-bp N-terminus EcoRI/BamHI fragment from pA-ALF1_1-706 (36) into pBluescript SK+.pBS-ITF2 was similarly made by ligating a 1,200-bp N-terminalHindIII/XbaI fragment from pCMV-ITF2 into pBluescript SK+. A 600-bpSmaI/HindIII fragment from pALF2 (36) encoding the E2A 3' untranslatedregion was ligated into pBluescript SK+ to make pBS-E2A. The vectorspCMV-ITF2 (8), pE-ALF1_1-70624 (36), pCMV-Mash2 and p $beta$ Actin-LacZ(12), p2E MCK-CAT (23), pT7-N3 (3), pHis-Mash2 (33),pGAL4-Hand1, pGAL4-Hand1 $Delta$ b, and pGAL4-Hand1 $Delta$ bHLH (19) have beenpreviously described. pCMV-Hand1, pCMV-Hand1 $Delta$ b (12-amino-acidbasic domain deleted), and pCMV-Hand1 $Delta$ bHLH (bHLH domain deleted)were constructed by inserting the EcoRI/XbaI fragment from theappropriate pGAL4 fusion vector into pcDNA-1 (Invitrogen). pCMV-VP16Hand1,encoding an N-terminal fusion of the VP16 acidic activation domainto HAND1, was made by ligating the VP16 activation domain (pBS-VP16mSna[33] BamHI/EcoRI fragment) and an EcoRI/XhoI mouse Hand1 cDNAfragment into pcDNA-1. pCMV-FLAGHand1 was constructed by ligatingan NdeI (filled-in)/XhoI fragment encoding an N-terminal FLAGepitope-tagged mouse HAND1 (FL-HAND1) into pcDNA3 (Invitrogen).pSV-E47 was made by ligating a HindIII/BamHI human E47 cDNA intopSV2 (Clontech). The glutathione S-transferase (GST)-HAND1 fusionvector pGST-HAND1 was made by inserting an EcoRI/XhoI ovine Hand1cDNA fragment into pGEX-3X (Pharmacia). The polyhistidine fusionbacterial expression vectors pHis-E47, pHis-Hand1, pHis-ALF1,pHis-ITF2, pHis-c-jun, and pHis-Id-2 were produced by ligatingthe following fragments into pHK (33): EcoRI from pT7-N3 (3),EcoRI of murine Hand1, KpnI/HindIII of human ALF1, ScaI/HindIIIfrom pCMV-ITF2, EcoRI of c-jun (includes the basic leucine zipperdomain), and KpnI/SalI of human Id-2. pT7FL-Hand1 $Delta$ N, a bacterialexpression vector which encodes a truncated (lacking the sequenceN terminal to the bHLH domain) ovine HAND1, was constructed byreplacing the E47 cassette in pT7-N3 with a SmaI/BamHI Hand1 fragment.The luciferase reporter constructs pL8G5-Luc and pL8E6-Luc werederived from pL8G5-CAT and pL8E6-CAT (19).

RNA in situ hybridization of histological sections. E8.5 conceptuses and E10.5 and 12.5 placentas were fixed with 4% paraformaldehyde. Tissues were embedded in paraffin, sectioned,and subjected to RNA in situ hybridization as previously described(30). Antisense ³³P-labeled riboprobes were prepared by using an RNA transcriptionkit (Stratagene). For ALF1, ITF2, and E2A probes, plasmids pBS-ALF1B,pBS-ITF2, and pBS-E2A were used. Probes specific to the placentallactogen 1 gene (Pl1) (21), Tpbp (previously called 4311) (28),Hand1 (12), and Mash2 (18) have been previouslydescribed.

Whole-mount in situ hybridization. Whole-mount in situ hybridization was performed for the Pl1 gene on Hand1 heterozygotes and Hand1, Mash2, and Hand1/Mash2mutants dissected out of the uterus at E8.5 (E0.5 is defined asnoon of the day on which vaginal plugging was detected). Decidualswellings were split longitudinally from the mesometrial to theantimesometrial end. The embryo and visceral yolk sac were removed,leaving the ectoplacental cone, chorion, Reichert's membrane,and trophoblast giant cell layer intact within the decidua. Deciduawere then processed as for E10.5 embryos (9). Digoxigenin-labeledPl1 probe was prepared by using digoxigenin labeling mix (BoehringerMannheim) and detected by using an anti-digoxigenin-alkaline phosphataseconjugate (Boehringer Mannheim). The resulting Pl1-positive trophoblastgiant cells (within the decidua) were photographed. DNA was preparedfrom the embryo proper and used for genotype analysis with PCRprimers specific to Hand1 and Mash2 as previously described (38,41).

Whole-mount $beta$ -galactosidase staining. E8.5 decidual swellings from Hand1 +/ $-$ ; Mrj +/6AD1 $beta$ geo × Hand1 +/ $-$ crosses were dissected as for whole-mount in situ hybridization.Decidua were then processed and subjected to staining for $beta$ -galactosidaseactivity as previously described (20). DNA was prepared fromthe embryo proper and used for genotype analysis with PCR primersspecific to Hand1 as previously described (38).

Coimmunoprecipitations. In vitro transcription-translation was performed with the Promega T_NT rabbit reticulocyte lysate kit and plasmids pT7-N3 (forFL-E47), pT7FL-Hand1 $Delta$ N, pHis-Hand1, pHis-Mash2, pHis-E47, andpT7-c-jun according to the manufacturer's instructions. Proteinswere labeled via the addition of [³⁵S]methionine to the reaction. Proteins were made in separate reactionsand then mixed for 30 min at 4°C in dilution buffer (100 mM NaCl,50 mM Tris [pH 7.5], 1 mM EDTA, 0.5% Triton X-100) in the presenceof protein A/G-agarose (Santa Cruz). Anti-FLAG antibody M2 (IBI)was then added to the supernatant, followed by an overnight incubationat 4°C. Agarose beads were washed five times with dilution buffer,resuspended in sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE) loading buffer, boiled, and subjected to SDS-PAGE.Gels were washed in Enhance (NEN), allowing the detection of labeledproteins byfluorography.

Cell culture and transfection. C3H10T1/2 fibroblasts were maintained in Dulbecco modified Eagle medium containing 10% fetal bovine serum (HyClone) plus 50µM $beta$ -mercaptoethanol (Gibco BRL). Rcho-1 cells were cultured inNCTC-135 medium (Sigma) supplemented with 20% serum, 50 µM $beta$ -mercaptoethanol,and 1 mM sodium pyruvate as previously described (12, 16).For reporter assays, C3H10T1/2 cells were transiently transfectedby using Lipofectamine (Gibco BRL) as previously described (33).Rcho-1 cells were transfected 5 h postplating, using LipofectaminePLUS (Gibco BRL), with fresh medium added 5 h posttransfection.Plasmid mixtures consisted of 100 ng of p $beta$ Actin-LacZ, 400 ng ofreporter plasmid (p2E MCK-CAT, pL8G5-Luc, or pL8E6-Luc), and expressionvector (with empty vector used to a total of 1 µg of DNA/35-mm-diameterwell). Cells were harvested 48 h posttransfection. Chloramphenicolacetyltransferase (CAT) levels were measured by enzyme-linkedimmunosorbent assay using a CAT ELISA kit (Boehringer Mannheim),while luciferase activity was assayed with D( $-$ )-luciferin (BoehringerMannheim) and an LB 9501 luminometer (Berthold). Values were normalizedto $beta$ -galactosidase activity (measured as described in reference45) and are reported as the mean ± standard error (SE) relativeto a value of 1.0 for empty expression vector alone. Transfectionswere performed in duplicate, with each experiment repeated threeto six times. Significant differences between values were determinedby analysis of variance followed by Student-Newman-Keulstest.

For giant cell differentiation assays (Fig. 6C), Rcho-1 stem cells were transfected by using Lipofectamine PLUS (Gibco BRL)5 h after plating to coverslips; 100 ng of p $beta$ Actin-LacZ and 500ng of expression vector were added per 35-mm-diameter well. Cellswere fixed 48 h posttransfection and stained for $beta$ -galactosidaseactivity (45). Giant cell differentiation was scored as theproportion of $beta$ -galactosidase-positive cells which had assumeda trophoblast giant cell morphology (12). Percent giant celldifferentiation values represent the mean ± SE for approximately250 cells per treatment group and were similar in two separateexperiments. For Mash2 titration experiments (Fig. 6A and B),Rcho-1 cells were transfected as described above, fixed in 4%paraformaldehyde, and permeabilized with methanol. Following incubationwith mouse anti-FLAG (1/200 dilution; IBI) and rabbit anti- $beta$ -galactosidase(1/400 dilution; Cappell) primary antibodies and anti-mouse-fluoresceinisothiocyanate and anti-rabbit-tetramethyl rhodamine isothiocyanate(1/50 dilution; Sigma) secondary antibodies, cells were stainedwith bisbenzimide and examined by fluorescence microscopy. Giantcell differentiation was scored as the percentage of tetramethylrhodamine isothiocyanate-positive cells which had the enlargednuclei characteristic of trophoblast giant cells. Results representthe mean ± SE of 25 fields examined for each treatment group,using a 40×objective.

Electrophoretic mobility shift assays. In vitro transcription-translation reactions were carried out as described above, with plasmids pHis-ALF1, pHis-ITF2, andpHis-Id-2 used to produce ALF1, ITF2, and ID-2, respectively.GST and GST-HAND1 were produced in Escherichia coli DH5 $alpha$ , usingthe plasmids pGEX-3X and pGST-HAND1, and batch purified by usingglutathione-Sepharose as instructed by the manufacturer (Pharmacia).Control (no DNA) reaction product was added to equalize the amountof reticulocyte lysate present in each lane. Proteins were preincubatedfor 15 min at 37°C prior to the addition of 10,000 cpm of ³²P-labeled probe (labeled via fill-in reactions [45]). Followingan additional 20 min at room temperature, reactions were resolvedvia electrophoresis on 5% nondenaturing acrylamide gels. For competitionexperiments, a 200-fold excess of unlabeled oligonucleotide wasadded prior to the first incubation step. Double-stranded oligonucleotidesused have all been previously described (33).

	RESULTS

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Overlapping expression of Hand1 and Mash2 in trophoblast subpopulations. RNA in situ hybridization on serial histological sections from E8.5 murine conceptuses demonstrated that Hand1 and Mash2 expressionoverlaps in the ectoplacental cone (Fig. 1F and G), a trophoblastsubpopulation which also expresses Tpbp (Fig. 1H). Hand1 expressionwas also detected in both primary and secondary trophoblast giantcells (Fig. 1B, I, and M), which were identified by their expressionof Pl1 (Fig. 1E and L). In contrast, Mash2 transcripts were notdetectable in giant cells (Fig. 1C, J, and N) but were presentat high levels in the chorion, where Hand1 expression was undetectable(compare Fig. 1F and G, arrows). At E10.5 and E12.5, placentalexpression of Hand1 had expanded to encompass all three trophoblastlayers: the outer layer of trophoblast giant cells, the spongiotrophoblastlayer, and the inner labyrinthine layer (Fig. 1I and M). However,Hand1 and Mash2 (Fig. 1J and N) hybridization signals were notuniformly detected in the labyrinthine and spongiotrophoblastlayers (Fig. 1K), with Mash2 signals limited to an even more restrictedportion of the spongiotrophoblast layer by E12.5 (Fig. 1N). Asan overlap in Hand1 and Mash2 expression was detected, we concludedthat their activities were not segregated based on distinct expressionalone. This suggested that their encoded protein products mightinteract in intermediate trophoblast subpopulations in vivo.

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FIG. 1. Hand1 and Mash2 have intersecting expression domains in trophoblast. (B to E) Serial sections of an E8.5 implantation site following RNA in situ hybridization with antisense probes for Hand1 (B), Mash2 (C), Tpbp (D), and Pl1 (E) shown in dark field. (A) Section B shown in light field. Hand1 and Mash2 expression overlaps in cells of the ectoplacental cone. (F to H) Increased magnification of panels B to D in boxed area depicted in panel A. Arrows indicate the chorion. (I to L) Expression of Hand1 (I), Mash2 (J), Tpbp (K), and Pl1 (L) in E10.5 placenta. (M and N) Expression of Hand1 (M) and Mash2 (N) in E12.5 placenta. (A to E) Panels I to N at ×50 magnification. Ch, chorion; EPC, ectoplacental cone; Lab, labyrinthine layer; Sp, spongiotrophoblast layer.

Restricted expression of E factors in trophoblasts. The function of many bHLH factors is dependent on their dimerization with one of the more widely expressed bHLH E factors(6, 26, 31). We examined the trophoblast expression ofthe three E-factor genes ALF1 (HEB, ITF1 [36]), E2A (E12/E47[53]), and ITF2 (ME2 [47]), using RNA in situ hybridization.Placental expression of E2A could not be detected between E8.5and E12.5 except in blood cells (Fig. 2D and data not shown).At E8.5, ALF1 and ITF2 transcripts localized to the embryo proper(not examined further), as well as to trophoblast cells of thechorion and ectoplacental cone (Fig. 2B and C). However, theywere not detectable in trophoblast giant cells. In contrast toMash2, expression of ALF1 and ITF2 did not extend to the limitsof the ectoplacental cone (Fig. 2G to I, dotted lines) and wasundetectable in the outer region where Tpbp was expressed (compareto Fig. 1H). By E10.5, transcripts of ALF1 and ITF2 remained undetectablein Pl1-positive trophoblast giant cells (Fig. 2J to M). Expressionof ALF1 was evident throughout the spongiotrophoblast and labyrinthinelayers (Fig. 2J), while that of ITF2 was nonuniform in the spongiotrophoblastlayer (Fig. 2K) in a manner similar to that of Mash2 (Fig. 1J).These studies therefore defined a subpopulation of trophoblastcells that coexpress the E-factor genes ALF1 and ITF2, along withHand1 and Mash2. Intriguingly, E-factor gene expression was undetectablein giant cells (both primary and secondary) at all stages examined.

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FIG. 2. E-factor gene expression during trophoblast development. (A to F) Serial sections of an E8.5 implantation site hybridized with antisense probes specific to ALF1 (B), ITF2 (C), E2A (D), Hand1 (E), and Mash2 (F) shown in dark field. (A) Section B shown in light field. E-factor gene expression is undetectable in trophoblast giant cells. (G to I) Magnification of boxed area shown in panel A for Mash2 (G), ALF1 (H), and ITF2 (I) probes. Note that ALF1 and ITF2 expression does not extend to the periphery of the ectoplacental cone (dotted line). (J to M) Serial sections of E10.5 placenta hybridized with probes for ALF1 (J), ITF2 (K), Pl1 (L), and Hand1 (M). Hand1 is expressed in Pl1-positive giant cells (bounded by the dotted line). (A to G) Panels J to M at ×5 magnification. Ch, chorion; E, embryo; EPC, ectoplacental cone; Lab, labyrinthine layer; Sp, spongiotrophoblast layer.

HAND1 can both homodimerize and heterodimerize with E factors. The colocalization of E-factor, Hand1, and Mash2 gene expression in the ectoplacental cone raised the possibility that theirprotein products could interact in vivo. The dimerization of HAND1and MASH2 with E factors has been previously analyzed by a numberof techniques (12, 19, 23). Coimmunoprecipitation assayswere performed with in vitro-translated proteins to determineif other interactions could occur. Both HAND1 and MASH2 were coprecipitatedwhen FL-E47 was used as the bait protein, while the negative control,c-Jun, was not (Fig. 3A). Using FL-HAND1 lacking the N terminus(FL-HAND1 $Delta$ N) as the bait, E47, but not MASH2, was coprecipitated(Fig. 3A). As both HAND1 and MASH2 coprecipitated with FL-E47in the same assay, we conclude that HAND1-MASH2 heterodimers donot readily form. Interestingly, full-length HAND1 was also coprecipitatedby FL-HAND1 $Delta$ N (Fig. 3A; note that His-HAND1 in vitro translationyields two bands). Compared to E47, a relatively small fractionof the total His-HAND1 was coprecipitated in this assay, suggestingthat the affinity of the HAND1-HAND1 interaction in vitro wasless than that of HAND1-E47 interaction.

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FIG. 3. HAND1 can both homodimerize and heterodimerize with E factors. (A and B) Coimmunoprecipitation assays using in vitro-translated FL-E47 or FL-HAND1 $Delta$ N as bait for untagged HAND1, MASH2, E47, and c-Jun. (A) Proteins were mixed and subjected to SDS-PAGE; (B) mixed proteins were immunoprecipitated (IP) with anti-FLAG antibody M2, washed, and resolved by SDS-PAGE. (C and D) Two-hybrid assays. The pL8G5-Luc reporter, in which luciferase expression is driven by a minimal promoter and five copies of the GAL4 upstream activation sequence DNA-binding site, was used along with 100 ng of the indicated GAL4 fusion construct. Different superscripts indicate statistically significant differences (P < 0.05).

To determine if these interactions could also occur in cells, two-hybrid assays were performed. An expression construct encodingHAND1 fused to the GAL4 DNA-binding domain (GAL4-HAND1) was usedto allow recruitment of HAND1 to GAL4 binding sites located upstreamof a luciferase reporter. In C3H10T1/2 fibroblasts, transfectionof GAL4-HAND1 and GAL4-HAND1 $Delta$ b (basic domain deleted) expressionconstructs stimulated reporter activity 25- and 50-fold, respectively.However, transfection of GAL4-HAND1 $Delta$ bHLH (bHLH domain deleted)had no significant effect on luciferase activity (Fig. 3C). Therefore,GAL4-HAND1 transcriptional activity was dependent on the HLH dimerizationdomain, likely due to recruitment of endogenous E factors whichcontain strong activation domains (37). Consistent with thisobservation, cotransfection of the E factor ITF2 potentiated GAL4-HAND1(wild type and $Delta$ b)-mediated activation a further fourfold. Thiseffect was likely due to dimerization with GAL4-HAND1, as luciferaseactivity was not affected by cotransfection of ITF2 when the GAL4-HAND1 $Delta$ bHLHmutant was used as bait (Fig. 3B).

In Rcho-1 rat trophoblast cells, transfection of GAL4-HAND1 stimulated reporter activity 2.5-fold (Fig. 3B), a modest levelrelative to that observed in C3H10T1/2 cells. Transfection ofITF2 potentiated GAL4-HAND1-mediated activation a further 2.5-fold.Wild-type HAND1 abolished GAL4-HAND1 activity, presumably by inhibitingthe dimerization of GAL4-HAND1 with E factors. Significantly,transfection of a VP16 activation domain-HAND1 fusion increasedGAL4-HAND1 activity 1.5-fold, with this effect being reproducibleover a number of experiments. This most likely reflects HAND1homodimerization, as VP16-HAND1 had no effect when GAL4-HAND1 $Delta$ bHLHwas used as the bait in this assay (data not shown). The VP16-HAND1fusion construct activated transcription 100-fold when pGAL4-ITF2was used as the bait, confirming that VP16-HAND1 was functional(data not shown). Therefore, these results demonstrate that HAND1homodimerization can occur in trophoblast cells. The ability ofHAND1 to homodimerize appeared to vary with cell type, as it wasnot detected in C3H10T1/2 cells (data notshown).

HAND1 inhibits MASH2 binding to E-box sequences. In electrophoretic mobility shift assays, MASH2 binds to canonical E-box sequences (CANNTG), such as the muscle creatine kinase(MCK) E-box (CACCTG), as a heterodimer with the E factors E47,ALF1, and ITF2 (Fig. 4A) (23). Transfection assays were performedin C3H10T1/2 fibroblasts in which a CAT reporter was regulatedby two copies of the MCK E box. The MASH2 activity observed waspresumably due to binding of heterodimers formed with endogenousE factors present in the cell, as the coaddition of low amountsof ITF2, ALF1, and E47 stimulated transcription with synergisticeffects (Fig. 4B). We tested the specificity of this binding incompetition assays. An excess of unlabeled oligonucleotides containingMCK and AP-4 (CAGCTG) E-box sequences abolished binding. Whileno competition was evident when non-E-box sequences were used,partial inhibition was observed when binding sites for Scleraxis(CATGTG [14]) and HAND1 (CATCTG [19]) were added (Fig. 4A).

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FIG. 4. HAND1 inhibits MASH2 binding to MCK E boxes by titrating E factors. (A and C) Electrophoretic mobility shift assay using a labeled MCK E-box probe. For indicated reactions, in vitro-translated FL-E47 (2 µl), His-MASH2 (4 µl), His-ALF1 (2 µl), and His-ITF2 (2 µl) were added. For competition assays, a 200-fold excess of unlabeled oligonucleotide was used. ns, nonspecific complex. (B and D) Transfection assays using C3H10T1/2 cells and the p2E MCK-CAT reporter, in which a CAT gene is driven by a minimal promoter and two copies of an MCK E-box sequence. Different superscripts indicate statistically significant differences (P < 0.05).

Unlike MASH2, GST-HAND1 binding to the MCK E box was not detected, either alone or in conjunction with the E factors E47 andALF1. However, the addition of GST-HAND1 inhibited E47-MASH2 bindingin a concentration-dependent manner (Fig. 4C). Similar resultswere obtained when E47-MASH2 dimers were formed prior to the additionof GST-HAND1 (data not shown). GST alone had no effect on E47-MASH2binding (Fig. 4C). As HAND1 forms heterodimers with E factorsbut not MASH2, this inhibition most likely reflected the formationof E47-HAND1, at the expense of E47-MASH2, dimers. Consistentwith this, HAND1 also inhibited binding of E47 and ALF1 homodimers(Fig. 4C). To further study the mechanism of HAND1 inhibition,transfection assays were performed with C3H10T1/2 fibroblastsand the MCK E-box reporter. Basal activity was stimulated 20-to 30-fold by cotransfection with the E factors ALF1 and ITF2and to a lesser (twofold) extent by MASH2 alone (Fig. 4D). Cotransfectionof HAND1 inhibited, in a concentration-dependent manner, the abilityof MASH2, ALF1, and ITF2 to stimulate transcription from the reporter.The basic domain, responsible for DNA binding, was not requiredfor this activity, as HAND1 $Delta$ b similarly inhibited MASH2 and ITF2(Fig. 4D and data not shown). However, deletion of the HLH domain(HAND1 $Delta$ bHLH) abolished HAND1-mediated inhibition. Therefore, whileunable to bind to the MCK subclass of E boxes, HAND1 can interferewith E-box-mediated transcription by forming heterodimers withE factors, thereby titrating the pool available for heterodimerizationwith other bHLH factors such asMASH2.

HAND1 and MASH2 bind competitively to a specific E-box sequence. E47-HAND1 complexes bind to DNA with the consensus sequence NNTCTG (Th1 boxes) (19). To further examine this, electrophoreticmobility shift assays were performed with a labeled Th1 E-boxoligonucleotide (CATCTG) as a probe. While E47 alone bound thissequence as a homodimer, the further addition of GST-HAND1 resultedin the formation of two new complexes. As partial cleavage ofthe GST moiety was evident in SDS-PAGE analysis of the purifiedGST-HAND1 preparation (data not shown), the mobilities of thesetwo complexes were consistent with those of E47-GST-HAND1 andE47-HAND1. Binding of these complexes was abolished by additionof the HLH factor ID-2, which dimerizes with E47 (2). GST-HAND1alone had no demonstrable binding activity at the concentrationsused in these assays. However, binding was evident at 100-fold-higherconcentrations (2 to 5 µg of protein), indicating that HAND1 homodimersmay also bind DNA (data not shown). To evaluate the DNA-bindingspecificity of the E47-HAND1 heterodimer, we performed competitionassays in which a large excess of unlabeled oligonucleotide wasadded. Of the sequences used, only the Th1 E box competed forbinding (Fig. 5A). E47-HAND1 therefore binds to Th1-box sequenceswith high specificity, not to related E-box sequences. Interestingly,these latter sequences included sites known to be bound by closebHLH relatives such as Scleraxis (1) and members of the Hairy/E(SPL)family, the latter of which share with HAND1 an atypical prolineresidue found in the basic domain.

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FIG. 5. HAND1 and MASH2 bind and activate transcription from a Th1 E-box sequence as heterodimers with E factors. (A) Electrophoretic mobility shift assay using a labeled Th1 E-box probe. For indicated reactions, 2 and 4 µl of in vitro-translated FL-E47 and His-MASH2, respectively, were used. For competition assays, a 200-fold excess of unlabeled oligonucleotide was used. ns, nonspecific complex. (B) Transfection assays using C3H10T1/2 fibroblasts. The pL8E6-Luc reporter, in which luciferase expression is driven by a minimal promoter and six copies of the Th1 E box, was used. Different superscripts indicate statistically significant differences (P < 0.05).

To determine if HAND1 could activate transcription from the Th1 E box, transfection assays were performed with C3H10T1/2 fibroblastsand a luciferase reporter regulated by six copies of this sequence.Transfection of a HAND1 expression vector stimulated transcriptionup to 30-fold in a concentration-dependent manner (Fig. 5B). Whilethese results were consistent within a given experiment, theywere observed in only three of six attempts. A variety of culturemodifications and different cell lots were tested, with similarresults. In negative experiments, a VP16-HAND1 fusion also failedto stimulate transcription (data not shown), whereas HAND1 inhibitionof ITF2-mediated activation was always observed (Fig. 4D). Thisindicates that the ability of HAND1-E-factor complexes to bindto Th1 E-box sequences may be regulated at a step followingdimerization.

The competition assays demonstrated that E47-MASH2 also bound to the Th1 E-box sequence with moderate affinity (Fig. 4A).We therefore wished to determine if HAND1 and MASH2 could competefor binding to the same DNA site. In electrophoretic mobilityshift assays, E47-MASH2 and E47-HAND1 dimers both bound to theTh1 E box (Fig. 5A). As the amount of GST-HAND1 added was increasedand that of MASH2 decreased, E47-MASH2 binding declined in favorof E47-HAND1 complexes (Fig. 5A). At intermediate concentrations,both complexes were evident (Fig. 5A). However, no novel complexeswere formed, indicating that E47-HAND1 and E47-MASH2 bind to asingle Th1 E box in a mutually exclusive manner. The predominantDNA-binding species therefore mirrors the relative concentrationsof MASH2 and HAND1. In transfection experiments, MASH2 stimulatedtranscription from the Th1 E-box reporter construct to levelscomparable to those observed for HAND1 (Fig. 5B). Therefore, MASH2and HAND1 can bind competitively to a shared subset of targetsequences.

Inhibition of Mash2 is not sufficient for Hand1 function in trophoblasts. To further examine the antagonistic activities of Hand1 and Mash2, giant cell differentiation assays were carried out withtransfected Rcho-1 trophoblast cells. Typically, 5 to 10% of Rcho-1cells in culture differentiate to trophoblast giant cells, a ratewhich is increased by overexpression of HAND1 (Fig. 6A) (12,25). We performed transfection experiments in which increasingamounts of an expression vector encoding MASH2 was cotransfectedwith a fixed amount of a FLAG-HAND1 construct. The ability ofFLAG-HAND1 to promote giant cell differentiation was inhibitedby the MASH2 expression construct in a concentration-dependentfashion (Fig. 6A). This effect was not due to a decrease in thelevels of FLAG-HAND1, as FLAG immunoreactivity was detected ina similar percentage of cells (Fig. 6B and data not shown). Incontrast to the effect of MASH2, the giant cell-promoting activityof FLAG-HAND1 was not inhibited by cotransfection of ITF2 (datanot shown). Therefore, as suggested by the biochemical data, therelative activities of HAND1 and MASH2 play a role in regulatinggiant cell differentiation.

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FIG. 6. Mutation of the HAND1 basic domain abrogates its ability to promote trophoblast giant cell differentiation. (A and C) Rcho-1 trophoblast cells were transiently cotransfected with a lacZ marker and the indicated expression vector(s). $beta$ -Galactosidase-positive cells were scored for giant cell morphology 2 days posttransfection. Different superscripts indicate statistically significant differences (P < 0.05). (B) Immunofluorescent detection of FL-HAND1 expression in transfected cells. Arrows and arrowheads indicate FL-HAND1-negative and -positive cells, respectively.

Based on its activities, the function of Hand1 in promoting giant cell differentiation could be mediated, at least in part,by the repression of MASH2-mediated transcription of target genesand/or Mash2 gene expression (38). To determine if the onlyfunction of Hand1 is to inhibit Mash2, Hand1/Mash2 double-mutantembryos were generated. If the major function of Hand1 in trophoblastwas to inhibit Mash2 expression and/or activity, the Hand1 mutantphenotype might be a consequence of ectopic Mash2 activity, whichis known to be sufficient to block giant cell differentiation(12, 25). In this case, the trophoblast defects of Hand1 mutantsshould be rescued by the further inactivation of Mash2. To examinetrophoblast giant cell differentiation, E8.5 implantation siteswere bisected and subjected to RNA in situ hybridization witha Pl1 probe. The perinuclear localization of Pl1 mRNA to the roughendoplasmic reticulum of trophoblast giant cells allowed an examinationof nuclear size. Strikingly, the nuclei of mural trophectodermcell derivatives surrounding the implantation site were significantlysmaller in Hand1 mutants (Fig. 7B), reflecting a failure for thesecells to increase in ploidy and indicating that giant cell transformationwas blocked. The number of Pl1-expressing cells was determined(Fig. 7C and D) as a measure of the number of trophoblast cellssurrounding each implantation site; the number reflects the derivativesof mural trophectoderm (primary giant cells) plus secondary giantcells that arise after implantation. Because Pl1 expression isreduced in mural trophectodermal derivatives in Hand1 mutants(Fig. 7C) (38), their numbers were independently assessed usingthe 6AD1 $beta$ geo (encoding $beta$ -galactosidase) allele of the Mrj gene(Fig. 7A), which is expressed in trophoblast giant cells (20).By either assessment, whereas wild-type implantation sites werelined by about 350 cells, mutants contained only about 80 cells.Strikingly, this low number is not significantly different fromthe number of mural trophectoderm cells found in the E4.5 blastocyst(10). The lower expression of Pl1, smaller nuclear size, anddecreased numbers of trophoblast cells lining the implantationsite observed in Hand1 mutants were all unaltered in Hand1/Mash2compound mutants (Fig. 7C and D). Therefore, Hand1 function introphoblast is not limited to restricting Mash2 expression and/oractivity.

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FIG. 7. Decreased mural trophectoderm cell number and nuclear size in Hand1 mutants is independent of Mash2 function. (A) $beta$ -Galactosidase staining for the 6AD1 $beta$ geo allele in E8.5 Hand1 +/ $-$ and $-$ / $-$ implantation sites. (B) High-magnification view of panel C showing mural trophoblast cells along the lateral side of the implantation site. Pl1 transcript localization is perinuclear. (C) E8.5 implantation sites derived from crosses between Hand1 +/ $-$ ; Mash2 +/ $-$ compound heterozygotes were bisected and subjected to whole-mount in situ hybridization using an antisense Pl1 probe. Shown is a low-magnification view of Pl1 expression in trophoblast giant cells in one-half of the implantation site. (D) Pl1-positive giant cells per conceptus were counted (three implantation sites per genotype).

The ability of Hand1 to promote giant cell differentiation regardless of its effect on Mash2 function could be mediated bytwo independent mechanisms: (i) indirectly, by inhibiting thedimerization of other bHLH factors, as yet unknown, with theirE-factor partners; and (ii) directly, by regulating the transcriptionof target genes when bound to Th1-box sequences. To discriminatebetween these activities, we tested the function of the HAND1basic domain mutant protein in transfected Rcho-1 cells. In contrastto wild-type HAND1, transfection of an expression vector encodingHAND1 $Delta$ b (DNA-binding basic domain deleted) had no significanteffect on giant cell differentiation relative to control (emptyexpression vector) (Fig. 6C). Importantly, the same HAND1 $Delta$ b mutantwas able to inhibit both E-factor- and MASH2-stimulated transcription(Fig. 4D), indicating that it is expressed and active in transfectedcells. These data suggest that in order to promote giant celldifferentiation, HAND1 does not solely inhibit the activity ofother bHLH proteins but also has a direct (DNA-binding) role inthisprocess.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Trophoblast giant cells develop throughout gestation due to the terminal differentiation of precursor cells present firstin the ectoplacental cone and later in the spongiotrophoblastlayer of the placenta. This process is regulated by bHLH transcriptionfactors encoded by the Hand1 and Mash2 genes, which have stimulatoryand repressive roles, respectively. We show here that Hand1 andMash2 expression patterns overlap in the ectoplacental cone andspongiotrophoblast but that Mash2 expression is down-regulatedas these trophoblast cell subpopulations differentiate into giantcells. The expression of the E-factor genes ALF1 and ITF2 is regulatedduring trophoblast development, as their expression is extinguishedin advance of giant cell differentiation. This finding has importantimplications for understanding both MASH2 and HAND1 function.First, the loss of E-factor partners should restrict MASH2 function,as E factors are essential DNA-binding partners for MASH2. Theexpression of other bHLH proteins (including HAND1) could alsoreduce MASH2 function by competing for dimerization with E factors.Second, HAND1 function could change during trophoblast differentiationdue to alterations in its DNA-binding specificity. In the ectoplacentalcone and spongiotrophoblast, HAND1 can associate with an E-factorbHLH protein, whereas in trophoblast giant cells, where the expressionof these factors was not detected, HAND1 presumably associateswith a different partner. The switching of dimerization partnerscould therefore lead to a different DNA-binding specificity, andas a result, the target genes to which HAND1 complexes bind wouldchange. Together, these data suggest that trophoblast differentiationis regulated by interactions between multiple bHLHproteins.

Three distinct expression domains of bHLH factors in the trophoblast lineage. Primary culture experiments have suggested that at least three functionally distinct trophoblast subpopulations exist in theE7.5-8.5 murine placenta (42, 43). Hand1 and Mash2 expressiondomains fit into these three trophoblast compartments: (i) thechorion, which expresses only Mash2; (ii) the ectoplacental cone,where Mash2 and Hand1 are coexpressed; and (iii) giant cells,where only Hand1 transcripts are present (summarized in Fig. 8).In intermediate trophoblast cells of the ectoplacental cone, theopposing activities of Hand1 and Mash2 clearly must be coordinated.Interestingly, our examination revealed that expression of E factors,the obligate dimerization partners of most bHLH factors, was alsosubject to regulation. Transcripts of ALF1 and ITF2 were localizedto the chorion and ectoplacental cone at E8.5, and to the labyrinthineand spongiotrophoblast layers at later periods, but remained undetectablein trophoblast giant cells at all stages. Strikingly, a more detailedanalysis revealed that expression of ALF1 and ITF2 was down-regulatedat the periphery of the ectoplacental cone (Fig. 8). As this occursprior to overt giant cell differentiation, it seems likely thattheir protein products are not present in giant cells. The absenceof an E-factor partner would be expected to effectively abolishMASH2 activity, thereby allowing giant cell differentiation tooccur.

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FIG. 8. Distinct bHLH compartments in early trophoblast development. Shown is a summary of expression patterns of bHLH factors and modifiers in trophoblast at E8.5. EPC, ectoplacental cone. Boxes: black, bHLH factors; dark gray, E factors; light gray, HLH factors; white, non-HLH factors.

The E-factor genes are widely considered to be ubiquitously expressed, although this belief primarily stems from whole-tissueNorthern blot and low-resolution in situ hybridization analysis(40, 53). Closer examination in the developing central nervoussystem revealed E-factor gene expression in proliferating neuroblastsand neurons at the initial stages of differentiation yet an absencein more mature, differentiated cells (8, 35, 47). Immunohistochemicalevaluation of E12/47 protein in a number of organs demonstratedthat expression is restricted primarily to proliferating or relativelyundifferentiated cells (44). Additionally, studies of ALF1 expressionin Schwann cells revealed a discordance between protein and transcriptlevels, with protein levels sharply down-regulated in terminallydifferentiated cells which continue to express abundant levelsof the mRNA (48). Therefore, the absence of E-factor gene expressionin trophoblast giant cells is generally consistent with findingsin other organs, where E-factor expression is down-regulated inadvance of terminaldifferentiation.

Expression of other bHLH factors in trophoblast has been described (Fig. 8). HES-2 and -3 are expressed in all trophoblastsubpopulations (32), while expression of Stra13 is restrictedto giant cells (4). The dominant-negative HLH genes Id-1 andId-2 are expressed in the chorion only (22). Overexpressionof ID-2 in Rcho-1 trophoblast inhibits giant cell differentiation,demonstrating a role for these factors in trophoblast development(12). In addition, non-bHLH modifiers of bHLH activity are alsoexpressed in trophoblast. The zinc finger transcription factorgene mSna, which inhibits giant cell differentiation in Rcho-1trophoblast cells, is expressed in the ectoplacental cone andspongiotrophoblast but is down-regulated during giant cell differentiation(33). Interestingly, mSNA binds to E-box sequences identicalto those bound by MASH2. I-mfa, first identified as an inhibitorof myogenic bHLH factors (7), is expressed in all three trophoblastlayers, and I-mfa mutants have a reduced number of trophoblastgiant cells. I-mfa binds to and inhibits MASH2 in vitro and promotesgiant cell differentiation in Rcho-1 cells (25). I-mfa can alsobind to HAND1 (25), although the functional consequences ofthis are unknown. The dynamic expression patterns of Hand1, Mash2,E-factor genes, and other regulators therefore define distinctbHLH environments present in the trophoblast subpopulations ofthe placenta (Fig. 8). Within each of these compartments, thebiochemical interplay between the different factors likely allowsprecise control over the relative actions of HAND1 andMASH2.

Multiple roles of Hand1 in trophoblast development. Hand1 mutant conceptuses show two distinct phenotypes in the trophoblast lineage. The most striking is that trophoblast giantcell differentiation is arrested at an early stage. Although thetrophoblast cell lineage is established in the mutants and theconceptuses implant normally, the derivatives of the mural trophectodermdo not undergo proper primary giant cell transformation, as theirnuclei remain relatively small (shown in this study). The enlargednuclei of giant cells reflect their increased DNA content dueto endoreduplication, i.e., continuous rounds of DNA synthesiswithout intervening mitoses (54). In addition, secondary giantcell differentiation does not occur, based on the failure of peripheralectoplacental cone cells to activate giant cell-specific genes(e.g., Pl1 and Limk) and to reduce ectoplacental cone-specificgenes (e.g., Mash2 and Tpbp) (38). Consistent with the latterdata, we demonstrated that the number of trophoblast cells surroundingHand1 mutant implantation sites at E8.5 (around 80) does not significantlydiffer from the number of mural trophectoderm cells present atthe expanded blastocysts stage (10). In addition to the giantcell phenotype, we have previously observed a phenotype in theectoplacental cone (38). Trophoblast cells of the ectoplacentalcone are precursors of secondary giant cells (43). Therefore,their numbers might be predicted to increase as a consequenceof a failure in secondary giant cell differentiation. However,the ectoplacental cones of Hand1 mutants are significantly smallerthan wild type (38). Therefore, while Hand1 mutant ectoplacentalcone cells are unable to undergo giant cell differentiation, theirproliferation and/or maintenance is also directly affected. Theprecise nature of this latter defect is unknown at present, thoughthe mutant ectoplacental cone cells continue to express the correctcell-specific genes (e.g., Tpbp, mSna, and Mash2) (38). Thefact that the number of giant cell precursors is not increasedin Hand1 mutants likely indicates that these cells are able toexit the mitotic cell cycle normally but cannot initiate the giantcell differentiation program. It is clear from our analyses, therefore,that Hand1 has distinct functions in two separate trophoblastsubpopulations. HAND1 likely regulates different genetic programsin these two trophoblast subpopulations. This suggests additionallevel(s) of regulation that determine the nature of HAND1 activityin a given celltype.

Regulation of distinct HAND1 activities. The combination of expression and biochemical data offers insight into how HAND1 could have distinct functions in the trophoblastlineage. In cells at the core of the ectoplacental cone, HAND1should predominantly form HAND1-E-factor heterodimers, which wouldpresumably regulate target genes involved in the proliferationand/or maintenance of these cells. At the periphery of the ectoplacentalcone, prior to secondary trophoblast giant cell differentiation,E-factor expression is down-regulated. Therefore, HAND1 likelypromotes giant cell differentiation, in the absence of E factors,as a dimer with a different bHLH partner. We found that HAND1can homodimerize in both coimmunoprecipitation and mammalian two-hybridexperiments. Alternatively, HAND1 may dimerize with a differentpartner. Among the bHLH factor genes studied, only Hand1, Stra13(4), and members of the HES (32) family are known to be expressedin giant cells. The precise nature of the complex functional ingiant cells is unknown at present. However, the switch in theHAND1 partner between the different trophoblast subpopulationscould alter its DNA-binding site specificity. The DNA target sequencesof bHLH factor dimers reflect the half-site binding specificitiesof the two proteins comprising the dimer complex. HAND1-E-factorheterodimers bind to NNTCTG sequences, representing the half-sitesequences bound by the HAND1 (NNT) and E-factor (CAG) molecules(19). Therefore, by switching in giant cells to a partner proteinwith a half-site specificity different from that of E factors,HAND1 could regulate the transcription of a different set of genes.This paradigm is observed with ARNT, which binds to differentDNA sequences in homodimeric versus heterodimeric complexes (49).This may represent a general mechanism through which bHLH factorscan have a spectrum of activities in subpopulations of one lineage.The promotion of homodimer formation only in more mature cellsmay help to ensure in earlier precursor cells that differentiationactivities incompatible with their development (e.g., onset ofthe endocyle) are repressed untilappropriate.

It is logical to predict that the lack of E-factor expression in giant cell precursors would facilitate a change in HAND1'sdimerization partner. However, it is not clear from our experimentsthat this down-regulation is actually required. A variety of othermechanisms aside from E-factor availability have been reportedto alter bHLH dimerization specificity (27, 29). Indeed wehave found that cotransfection of ITF2 does not block the abilityof HAND1 to promote giant cell differentiation (I. C. Scott, unpublishedresults). Further work will be required to scrutinize the predictionsof this model for HAND1 functions. Tethered bHLH dimers in whicha single polyprotein encodes the two bHLH proteins to be testedseparated by a flexible linker can be generated (34). As thesecomplexes are resistant to disruption by other HLH proteins presentin the cell, their use would permit dissection of the specificactivities of individual complexes (e.g., HAND1-E factor versusHAND1-HAND1) in trophoblast development. Transfection of trophoblaststem cell lines (51) derived from Hand1 mutants would providethe best system for examining theseactivities.

	ACKNOWLEDGMENTS

We thank N. Hattori, who made important contributions to the Rcho-1 differentiation experiments. A. Nagy provided Mash2 mutantmice. S. Hollenberg, T. Neuman, P. Jorgensen, and S. Fisher kindlyprovided plasmids. We also thank K. Harpal for his aid in histologyand tissuesectioning.

This work was supported by a grant from the Medical Research Council of Canada (to J.C.C.). I.C.S. was supported by a studentshipfrom the Natural Science and Engineering Research Council, P.R.was supported by a fellowship from the Wellcome Trust, and J.C.C.is a Scholar of the Medical Research Council ofCanada.

	FOOTNOTES

^* Corresponding author. Mailing address: Samuel Lunenfeld Research Institute, Rm. 880, Mount Sinai Hospital, 600 UniversityAve., Toronto, Ontario M5G 1X5, Canada. Phone: (416) 586-8261.Fax: (416) 586-8588. E-mail: cross{at}mshri.on.ca.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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32. Nakayama, H., Y. Liu, S. Stifani, and J. C. Cross. 1997. Developmental restriction of Mash-2 expression in trophoblast correlates with potential activation of the NOTCH-2 pathway. Dev. Genet. 21:21-30[CrossRef][Medline].

33. Nakayama, H., I. C. Scott, and J. C. Cross. 1998. The transition to endoreduplication in trophoblast giant cells is regulated by the Sna zinc-finger transcription factor. Dev. Biol. 199:150-163[CrossRef][Medline].

34. Neuhold, L. A., and B. Wold. 1993. HLH forced dimers: tethering MyoD to E47 generates a dominant positive myogenic factor insulated from negative regulation by Id. Cell 74:1033-1042[CrossRef][Medline].

35. Neuman, T., A. Keen, E. Knapik, D. Shain, M. Ross, H. O. Nornes, and M. X. Zuber. 1993. ME1 and GE1: basic helix-loop-helix transcription factors expressed at high levels in the developing nervous system and in morphogenetically active regions. Eur. J. Neurosci. 5:311-318[CrossRef][Medline].

36. Nielsen, A. L., N. Pallisgaard, F. S. Pedersen, and P. Jorgensen. 1992. Murine helix-loop-helix transcriptional activator proteins binding to the E-box motif of the Akv murine leukemia virus enhancer identified by cDNA cloning. Mol. Cell. Biol. 12:3449-3459[Abstract/Free Full Text].

37. Quong, M. W., M. E. Massari, R. Zwart, and C. Murre. 1993. A new transcriptional-activation motif restricted to a class of helix-loop-helix proteins is functionally conserved in both yeast and mammalian cells. Mol. Cell. Biol. 13:792-800[Abstract/Free Full Text].

38. Riley, P., L. Anson-Cartwright, and J. C. Cross. 1998. The Hand1 helix-loop-helix transcription factor is essential for placentation and cardiac morphogenesis. Nat. Genet. 18:271-275[CrossRef][Medline].

39. Rinkenberger, J., J. C. Cross, and Z. Werb. 1997. Molecular genetics of implantation in the mouse. Dev Genet. 21:6-20[CrossRef][Medline].

40. Roberts, V. J., R. Steenbergen, and C. Murre. 1993. Localization of E2A mRNA expression in developing and adult rat tissues. Proc. Natl. Acad. Sci. USA 90:7583-7587[Abstract/Free Full Text].

41. Rossant, J., F. Guillemot, M. Tanaka, K. Latham, M. Gertsenstein, and A. Nagy. 1998. Mash2 is expressed in oogenesis and preimplantation development but is not required for blastocyst formation. Mech. Dev. 73:138-191.

42. Rossant, J., and L. Ofer. 1977. Properties of extra-embryonic ectoderm isolated from postimplantation mouse embryos. J. Embryol. Exp. Morphol. 39:183-194[Medline].

43. Rossant, J., and W. Tamura-Lis. 1981. Effect of culture conditions on diploid to giant-cell transformation in postimplantation mouse trophoblast. J. Embryol. Exp. Morphol. 62:217-227[Medline].

44. Rutherford, M. N., and D. P. LeBrun. 1998. Restricted expression of E2A protein in primary human tissues correlates with proliferation and differentiation. Am. J. Pathol. 153:165-173[Abstract/Free Full Text].

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

46. Soares, M. J., B. M. Chapman, T. Kamei, and T. Yamamoto. 1995. Control of trophoblast cell differentiation: lessons from genetics of early pregnancy loss and trophoblast neoplasia. Dev. Growth Differ. 37:355-364[CrossRef].

47. Soosaar, A., A. Chiaramello, M. X. Zuber, and T. Neuman. 1994. Expression of basic-helix-loop-helix transcription factor ME2 during brain development and in the regions of neuronal plasticity in the adult brain. Brain. Res. Mol. Brain. Res. 25:176-180[Medline].

48. Stewart, H. J. S., G. Zoidl, M. Rossner, A. Brennan, C. Zoidl, K.-A. Nave, R. Mirsky, and K. R. Jessen. 1997. Helix-loop-helix proteins in Schwann cells: a study of regulation and subcellular localization of Ids, REB, and E12/47 during embryonic and postnatal development. J. Neurosci. Res. 50:684-701[CrossRef][Medline].

49. Swanson, H. I., W. K. Chan, and C. A. Bradfield. 1995. DNA binding specificities and pairing rules of the Ah receptor, ARNT, and SIM proteins. J. Biol. Chem. 270:26292-26302[Abstract/Free Full Text].

50. Tanaka, M., M. Gertsenstein, J. Rossant, and A. Nagy. 1997. Mash2 acts cell autonomously in mouse spongiotrophoblast development. Dev. Biol. 190:55-65[CrossRef][Medline].

51. Tanaka, S., T. Kunath, A.-N. Hadjantonakis, A. Nagy, and J. Rossant. 1998. Promotion of trophoblast stem cell proliferation by FGF4. Science 282:2072-2075[Abstract/Free Full Text].

52. Voronova, A., and D. Baltimore. 1990. Mutations that disrupt DNA binding and dimer formation in the E47 helix-loop-helix protein map to distinct domains. Proc. Natl. Acad. Sci. USA 87:4722-4726[Abstract/Free Full Text].

53. Watada, H., Y. Kajimoto, Y. Umayahara, T. Matsuoka, T. Morishima, Y. Yamasaki, R. Kawamori, and T. Kamada. 1995. Ubiquitous, but variable, expression of two alternatively spliced mRNAs encoding mouse homologues of transcription factors E47 and E12. Gene 153:255-259[CrossRef][Medline].

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54.	<