Critical Role of the HMGI(Y) Proteins in Adipocytic Cell Growth and Differentiation

doi:10.1128/MCB.21.7.2485-2495.2001

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Molecular and Cellular Biology, April 2001, p. 2485-2495, Vol. 21, No. 7
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.7.2485-2495.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Critical Role of the HMGI(Y) Proteins in Adipocytic Cell Growth and Differentiation

Rosa Marina Melillo,¹ Giovanna Maria Pierantoni,¹ Stefania Scala,¹ Sabrina Battista,¹ Monica Fedele,¹ Antonella Stella,² Maria Cristina De Biasio,³ Gennaro Chiappetta,³ Vincenzo Fidanza,⁴ Gianluigi Condorelli,⁴ Massimo Santoro,¹ Carlo M. Croce,⁴ Giuseppe Viglietto,³ and Alfredo Fusco²^,^*

Centro di Endocrinologia ed Oncologia Sperimentale del Consiglio Nazionale delle Ricerche, Dipartimento di Biologiae Patologia Cellulare e Molecolare, Facoltà di Medicina e Chirurgia, Università degli Studi di Napoli,¹ and Istituto Nazionale dei Tumori Fondazione Senatore Pascale,³ 80131 Naples, and Dipartimento di Medicina Sperimentale e Clinica, Facoltà di Medicina e Chirurgia di Catanzaro, Università degli Studi di Catanzaro, 88100 Catanzaro,² Italy, and Kimmel Cancer Center, Jefferson Medical College, Philadelphia, Pennsylvania 19107⁴

Received 2 June 2000/Returned for modification 31 July 2000/Accepted 11 January 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The high-mobility group I (HMGI) nonhistone chromosomal proteins HMGI(Y) and HMGI-C have been implicated in defining chromatinstructure and in regulating the transcription of several genes.These proteins have been implicated in adipocyte homeostasis:a severe deficiency of fat tissue is found in mice with targeteddisruption of the HMGI-C locus, and lipomagenesis in humans isfrequently associated with somatic mutations of HMGI genes. Theaim of this study was to examine the role of HMGI(Y) proteinsin adipocytic cell growth and differentiation. First, we foundthat differentiation of the preadipocytic 3T3-L1 cell line causedearly induction of HMGI(Y) gene expression. Suppression of HMGI(Y)expression by antisense technology dramatically increased thegrowth rate and impaired adipocytic differentiation in these cells.The process of adipogenic differentiation involves the interplayof several transcription factors, among which is the CCAAT/enhancer-bindingprotein (C/EBP) family of proteins. These factors are requiredfor the transcriptional activation of adipocyte-specific genes.We also tested the hypothesis that HMGI(Y) might participate intranscriptional control of adipocyte-specific promoters. We foundthat HMGI(Y) proteins bind C/EBP $beta$ in vivo and in vitro. Furthermore,we show that HMGI(Y) strongly potentiates the capacity of C/EBP $beta$ to transactivate the leptin promoter, an adipose-specific promoter.Taken together, these results indicate that the HMGI(Y) proteinsplay a critical role in adipocytic cell growth anddifferentiation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The mammalian high-mobility group I (HMGI) family of chromosomal proteins includes HMG-I and HMG-Y, which are coded for bythe same gene, HMGI(Y), through alternative splicing (23), andthe closely related HMGI-C protein (27). The HMGI proteins areinvolved in the regulation of chromatin structure and function(25). While not typical transcriptional activators, HMGI(Y)proteins are required for the expression of many eukaryotic genes.These proteins bind adenine- and thymine-containing sequenceslocated in the minor groove of DNA. Their DNA-binding domain islocated in the N-terminal region of the protein and contains threeshort basic repeats, the so-called AT hooks. HMGI(Y) DNA-bindingsites have been identified in many promoters, e.g., interleukin-4(13), interleukin-2 receptor $alpha$ -chain (22), lymphotoxin (15),and the human papovavirus JC (24) genes. These sites are oftenclose to the DNA-binding sites of known transcription factorslike NF- $kappa$ B (38) and Tst-1/Oct-6 (24) and appear critical forviral induction of the human beta interferon gene (14, 38,39). HMGI(Y) also interacts directly with several transcriptionfactors. In fact, it binds to the basic leucine zipper regionof the activating transcription factor 2, thus promoting its dimerizationand binding to the beta interferon promoter (14).

HMGI-C gene knockout mice show a pygmy phenotype with a reduction of the adult body weight, mainly affecting fat tissue (49).The fat index, a reliable indicator of the total fat content relativeto body weight, is approximately eight times lower in pygmy micethan in the wild-type littermates. Furthermore, the regulationof HMGI-C in vivo modulates obesity in a mouse model, and rearrangementsof the HMGI-C and the HMGI(Y) genes have been found in human lipomascarrying chromosomal translocations involving the regions 12q13-14and 6p21, respectively (2, 34, 40). Our group has recentlydemonstrated that the HMGI-C rearrangement plays a critical rolein the generation of lipomas. In fact, transgenic mice carryinga truncated HMGI-C gene, which contains only the three AT hookdomains, develop a giant phenotype and predominantly abdominaland pelvic lipomatosis (4). These observations, taken together,implicated HMGI(Y) proteins in adipogenesis. To elucidate furtherthe mechanism of action of HMGI(Y) in adipogenesis, we used mouse3T3-L1 fibroblasts as a model system. These cells differentiateinto adipocytes upon treatment with specific agents (35). Adipocytedifferentiation involves a group of transcription factors, CCAAT/enhancer-bindingproteins (C/EBPs) (5, 29, 33, 42, 46), which are expressedat specific stages of adipogenesis. Hormonal stimulation causesC/EBP $beta$ and C/EBP $delta$ levels to increase and induce the expressionof the transcription factor peroxisome proliferator-activatedreceptor gamma (44). This factor, in turn, leads to an increaseof C/EBP $alpha$ , which promotes the induction of several adipocyte-specificgenes, including that for the fatty acid-binding protein 422/aP2(11, 12) and the obese gene, which encodes leptin (21).Here we report the following: (i) HMGI(Y) gene expression increasesduring adipocytic conversion of 3T3-L1 cells; (ii) blockage ofHMGI(Y) synthesis stimulates cell growth and impairs 3T3-L1 differentiation;(iii) HMGI(Y) physically interacts with C/EBP $beta$ in vivo and invitro; and (iv) HMGI(Y) proteins greatly enhance the C/EBP $beta$ -mediatedtransactivation of the leptinpromoter.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cell culture, transfections, and plasmids. The mouse NIH 3T3-L1 cells used in this study were generously donated by E. Santos (National Cancer Institute, National Institutesof Health, Bethesda, Md.). Cell cultures were grown in Dulbecco'smodified Eagle's medium (DMEM) supplemented with 10% calf serum(GIBCO BRL, Life Technologies, Gaithersburg, Md.). Induction ofadipocytic differentiation in 3T3-L1 cells was performed essentiallyas described elsewhere (35). Briefly, confluent 3T3-L1 cellswere grown in DMEM supplemented with 10% calf serum until confluencywas reached. Two days later, they were grown in DMEM supplementedwith 10% fetal calf serum, 0.5 mM 1-methyl-3-isobutylxanthine,10⁶ M dexamethasone, and 10 µg of insulin/ml for 48 h. Cells werefurther cultured in the same culture medium devoid of dexamethasoneand methylisobutylxanthine for 6 days. The 3T3-L1 fibroblastswere transfected by the calcium phosphate technique (18). Transfectedcells were subjected to G418 selection (400 µg/ml). 293 cellswere maintained in DMEM medium containing 10% fetal calf serum(GIBCO BRL, Life Technologies) and transiently transfected forin vivo binding assays or luciferase assays as described above.A 1,500-bp cDNA including the HMGI(Y) gene was subcloned intothe HindIII site of the expression vector pRc/CMV (Invitrogen).A 489-bp cDNA fragment corresponding to the entire coding sequenceof the HMGI(Y) gene was subcloned into the HindIII and XbaI sitesof the expression vector pRc/CMV (Invitrogen) in the antisenseorientation. Expression of the sense and antisense HMGI(Y) RNAwas achieved by reverse transcription (RT)-PCR: the forward primerfor the sense vector, designed on the ATG sequence of the HMGI(Y)gene, was as follows: 5'-AGGAGAATGAGCGAGTCG-3'. The reverse primer,designed on the Sp6 sequence of the cytomegalovirus (CMV) vector,was as follows: 5'-AGTCGAGGCTGATCAGCGAG-3'. The forward primerfor the antisense vector, designed on the stop codon sequenceof the HMGI(Y) gene, was as follows: 5'-CTGCGAGTGGTGATCACT-3'.The reverse primer, designed on the Sp6 sequence of the CMV vector,was as follows: 5'- AGTCGAGGCTGATCAGCGAG-3'. The p( $-$ 161)ob-lucplasmid, containing 161 bp of the obese gene promoter drivinga luciferase gene, and the m52 mutant, in which the C/EBP bindingmotif has been disrupted, are also described elsewhere (20).

Growth curves. For standard growth curves, cells were seeded at a density of 10⁵ in 60-mm-diameter plates (Falcon) and grown in DMEM supplementedwith 10% calf serum (GIBCO). Medium was renewed every 2 days,and cells were counted (see Fig. 4A). The doubling time was measuredwhen the cells were in the logarithmic phase of growth: for 3T3-L1and 3T3-L1-HMGI(Y)s cells, it occurred between days 3 and 4, andfor 3T3-L1-HMGI(Y)as cells, it occurred between days 4 and 5 ofculture. For growth curves of differentiating cells, cells wereseeded and grown as described above until confluent. Two daysafter reaching confluence, cells were induced to differentiateaccording to the standard protocol (see above). Starting from1 day after induction of differentiation, cells were counted (seeFig. 4B).

Northern blot analysis. Total RNA was extracted with RNAzol (Tel-Test, Inc., Friendswood, Tex.) according to standard procedures (32). Northernblotting and hybridizations were carried out as previously described(32). The HMGI probe was derived from pHMGI(Y) (23). A 0.4-kbEcoRI-HindIII fragment corresponding to the cDNA of the constitutivelyexpressed enzyme human glyceraldehyde-3-phosphate dehydrogenase(GAPDH) was used to control equal RNA loading. Quantificationof the hybridization signal was performed using a Molecular DynamicsPhosphorImager. The images recorded by the PhosphorImager wereanalyzed by volume integration with the ImageQuantsoftware.

RT-PCR analysis of the expression of the adipocyte differentiation markers. Total RNA, digested with DNase, was reverse transcribed using random exonucleotides as primers (100 mM) and 12 U of avianmyeloblastosis virus reverse transcriptase (GIBCO). SubsequentPCR amplification was as follows: 200 ng of cDNA was amplifiedin a 25-µl reaction mixture containing Taq DNA polymerase buffer,0.2 mM deoxynucleoside triphosphates, 1.5 mM MgCl₂, 0.4 mM concentrationsof each primer, and 1 U of Taq DNA polymerase (Perkin-Elmer-Cetus,Branchburg, N.J.). The PCR amplification was performed for 30cycles (94°C for 30 s, 55°C for 2 min, and 72°C for 2 min). Theprimers used for aP2 gene expression were 5'-GATGTCAGCAGGAAGTCACC-3'and 3'-CGAAGGAGGTTTAGCAAGAG-5', corresponding to nucleotides 109to 138 and nucleotides 427 to 408 (41). For the obese gene expressionthe sequences of the primers used were 5'-CCTGCTCCAGCAGCTGCAAG-3'and 5'-GAGGAAAATGTGCTGGAGACCC-3', which map on exon 1 and exon2, respectively, and give rise to a specific 195-bp product (20).In addition, a set of primers specific for GAPDH was added toeach reaction after 20 cycles of PCR to serve as an internal controlfor the amount of cDNA tested. The GAPDH-specific primers werethe following: 5'-ACATGTTCCAATATGATTCC-3' (forward), correspondingto nucleotides 194 to 214, and 5'-TGGACTCCACGACGTACTCAG-3' (reverse),corresponding to nucleotides 336 to 356. The reaction productswere analyzed on a 2% agarose gel and then transferred by blottingto GeneScreen Plus nylon membranes (Dupont, Boston, Mass.). Themembranes were hybridized with an HMGI(Y) cDNA probe (7, 23).The relative levels of aP2 and ob expression were assessed bycomparison with the level of GAPDH in the samesample.

Immunoblotting and immunoprecipitation. Protein extracts were prepared from terminally differentiated or undifferentiated fibroblasts as previously described (6).The following antibodies were used for immunoprecipitation andWestern blotting: anti-C/EBP $beta$ (C-19) rabbit polyclonal antibodies(Santa Cruz Biotechnology, Santa Cruz, Calif.) and anti-HA 12CA5mouse monoclonal antibodies (Boehringer, Mannheim, Germany). Therabbit polyclonal antibodies directed against the HMGI(Y) proteinsalready have been described (7, 8). For Western blot experiments,equal amounts of protein lysates were loaded, as demonstratedby staining of the membranes with Ponceau Red. To confirm equalloading, the same Western blots were incubated with antibodiesto $gamma$ -tubulin (Sigma-Aldrich Corporation, St. Louis, Mo.). Forcoimmunoprecipitation experiments, antigens and antibodies wereincubated for 1 h before the addition of protein A-Sepharose beads(Pharmacia Biotech, Uppsala, Sweden). After another 1 h, the beadswere collected and washed five times with lysis buffer. The beadswere then boiled in sodium dodecyl sulfate (SDS) loading bufferfor immunoblotting analysis. The protein extracts separated bySDS-polyacrylamide gel electrophoresis (SDS-PAGE) were transferredto Immobilon-P transfer membranes (Millipore). Membranes wereblocked with 5% nonfat milk proteins and incubated with antibodiesat the appropriate dilutions. Bound antibodies were detected bythe appropriate horseradish peroxidase-conjugated secondary antibodiesfollowed by enhanced chemiluminescence(Amersham).

In vitro and in vivo binding assays. For in vitro binding assays, the HMGI(Y) cDNA was expressed as a glutathione S-transferase (GST) fusion protein in bacteriaas described previously (10). Briefly, a 900-bp EcoRI-BamHIfragment generated by PCR and including the complete coding sequencewas subcloned in pGEX2T. The GST-HMGI(Y) construct was used totransform Escherichia coli strain BL21. Bacterially expressedGST and GST-HMGI(Y) proteins were bound to glutathione-agarose(Sigma-Aldrich Corporation). The beads were washed, and the sizeand purity of the bound protein were evaluated by Coomassie stainingof an SDS-polyacrylamide gel. Equal amounts of GST and GST-HMGI(Y)proteins (5 µg) were used for binding assays. C/EBP $beta$ cDNA wasobtained by PCR amplification and cloned in the pBluescript vector(Stratagene, La Jolla, Calif.). Transcription and translationreactions were performed with the T7-rabbit reticulocyte lysatekit (Promega, Madison, Wis.) as suggested by the manufacturer.The in vitro-translated C/EBP $beta$ was allowed to associate with glutathione-agarose-boundGST or GST-HMGI(Y) for 2 h in lysis buffer (6) at 4°C. Thepellets were washed four times in lysis buffer, and the proteinswere dissociated by boiling in loading buffer and electrophoresedon a 10% polyacrylamide-SDS gel. The proteins were transferredto Immobilon-P, and C/EBP $beta$ was visualized as described above.For in vivo binding assays, 293 cells were transfected as describedby Graham and van der Eb (18). Cells were transfected with 5µg of each plasmid, and carrier DNA was added to a total of 10µg. Cells were harvested 36 h after transfection, and proteinextracts were prepared as described above. Extracts were immunoprecipitatedand immunoblotted with the indicatedantibodies.

Transient transfection and luciferase activity assay. Transfections into 293 cells were performed by calcium phosphate precipitation (18). Cells were transfected with 5 µg ofp( $-$ 161)ob-luc, m52, or RSV-luc reporter plasmids together with1 µg of pHMGI(Y)s. The hemagglutinin (HA)-tagged HMGI(Y) wild-typeand deletion mutants were generated by PCR, sequenced, and subclonedinto the pCEFL vector. One microgram of pSV2CAT plasmid was cotransfectedto demonstrate equal transfection efficiency in the cell linestested, and chloramphenicol acetyltransferase activity was measuredby thin-layer chromatography with 95% chloroform-5% methanol.Cells were harvested 24 h after transfection, and luciferase activitywas measured with a luminometer (Lumat LB9507; Berthold). Therelative activities were calculated by dividing the normalizedactivities by the activity of the m52 and the Rous sarcoma virusconstructs, which were considered to be equal to 1. The data representthe average of results from three independent experiments, performedin duplicate, with standarddeviations.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

3T3-L1 adipocytic differentiation is associated with an increase in HMGI(Y) protein levels. We first investigated whether the expression of HMGI(Y) was regulated during adipocyte differentiation. As a model system,we used the 3T3-L1 preadipocytic cells, which have been extensivelycharacterized. These cells undergo adipocytic conversion uponexposure to fetal bovine serum and differentiating agents (dexamethasone,methylisobutylxanthine, and insulin), as previously described(35). Cells were harvested in growing, undifferentiated conditions,at time zero (2 days postconfluence), and at different times duringdifferentiation, and RNAs and proteins were prepared. Northernblot analysis showed that endogenous HMGI(Y) is expressed at lowlevels in growing cells, and it increases at time zero. It reachesits maximal level between 6 h and day 1 of treatment with differentiatingagents and decreases again at day 4 (Fig. 1A), suggesting thatthe expression of HMGI(Y) is regulated, during differentiation,at the mRNA level. Western blot analysis showed a parallel increaseof the HMGI(Y)-gene-specific protein product (Fig. 1B).

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FIG. 1. (A) HMGI(Y) induction during NIH 3T3-L1 preadipocyte differentiation. Total RNA (20 µg/lane) extracted from proliferating and differentiated 3T3-L1 cells was hybridized with the HMGI(Y) cDNA and then with a rat GAPDH probe as a control for RNA loading. RNA was extracted from undifferentiated proliferating cells (P) at time zero and at 6 h, 1 day, and 4 days of differentiation, as indicated. (B) Nuclear proteins extracted from normal and induced 3T3-L1 cells were separated (20 µg/lane) by SDS-PAGE and transferred to polyvinylidene difluoride membranes. Western blots were incubated first with antibodies specific for HMGI(Y) proteins and then with horseradish peroxidase-conjugated secondary antibodies; the immunocomplexes were detected by enhanced chemiluminescence. As a control for equal loading, the blotted proteins were stained with Ponceau Red. Moreover, the same Western blots were incubated with antibodies to the ubiquitous $gamma$ -tubulin protein. Proteins were extracted from the same cells as in panel A.

Inhibition of HMGI(Y) protein synthesis affects the differentiation and growth rate of 3T3-L1 cells. To investigate whether HMGI(Y) expression is a prerequisite for adipocytic differentiation, HMGI(Y) protein synthesis wassuppressed by an antisense methodology. To this aim, 3T3-L1 cellswere transfected with a plasmid carrying the HMGI(Y) gene in theantisense orientation (pCMV-HMGI-Yas) under the transcriptionalcontrol of the cytomegalovirus promoter (Fig. 2A). At the sametime, to investigate the effect of the overexpression of HMGI(Y)in the 3T3-L1 cells, we generated the 3T3-L1-HMGI(Y)s cells, carryingthe HMGI(Y) gene in the sense orientation [pCMV-HMGI(Y)s]. Theempty vector (pCMVneo) served as a control. Six 3T3-L1-HMGI(Y)asclones showing the lowest HMGI(Y) protein levels, four overexpressingHMGI(Y), and one mass population for each transfection were chosenfor further analyses. Cells transfected with the empty vector(four clones and a mass population) were used as a control forour experiments. A strand-specific RT-PCR assay showed the expressionof the sense and antisense HMGI(Y) mRNA in the transfected cells(Fig. 2B and B'). The HMGI(Y) protein levels were remarkably reducedin the 3T3-L1-HMGI(Y)as cells, whereas they were increased inthe 3T3-L1-HMGI(Y)s cells (Fig. 2C), compared with the parentaland the backbone-vector-transfected cells. As a positive controlfor HMGI(Y) expression, we used the PC MPSV cell line (rat thyroidcells transformed by the myeloproliferative sarcoma virus), whichexpresses high levels of the protein (9). The HMGI(Y)as cellsfailed to undergo adipocytic differentiation upon being givendifferentiating treatment. Adipocyte differentiation of 3T3-L1cells in culture is similar to the in vivo process, i.e., enlargedcells filled with lipid droplets and expressing adipocyte-specificgene products appear. As shown in Fig. 3A, the typical fat dropletsdid not appear in the cytosol of antisense-expressing cells followingdifferentiating treatment. We also analyzed the expression oftwo adipocyte-specific molecular markers, the adipocyte lipid-bindingprotein, aP2, and the product of the obese gene, leptin. To thisaim, we used a semiquantitative RT-PCR assay with parental, HMGI(Y)as,and pCMVneo 3T3-L1 cells. Upon differentiating treatment, inductionof the aP2 and leptin genes was suppressed in 3T3-L1-HMGI(Y)ascells but not in the parental and the pCMVneo-transfected 3T3-L1cells (Fig. 3B). When we analyzed the phenotype of the 3T3-L1-HMGI(Y)scells, we did not observe any differences from the parental orthe empty-vector-transfected 3T3-L1 cells (data not shown).

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FIG. 2. (A) HMGI(Y) sense and antisense constructs were generated as described in Materials and Methods. The untranslated region, DNA-binding domain, and acidic domain of the HMGI(Y) protein are indicated. (B) RT-PCR analysis of pHMGI(Y)s expression in 3T3-L1-HMGI(Y)s cells. The sources of RNAs are the following: lane 1, PCR on the pCMV-HMGI(Y)s plasmid (positive control); lanes 2, 3, and 4, 3T3-L1-HMGI(Y)s (cell clones 1, 2, and 3); lane 5, 3T3-L1 pCMVneo clone 1. (B') RT-PCR analysis of pHMGI(Y)as expression in 3T3-L1-HMGI(Y)as cells. The sources of RNAs are the following: lane 1, PCR on a pCMV-HMGI(Y)as plasmid (positive control); lanes 2, 3, and 4, 3T3-L1-HMGI(Y)as (cell clones 1, 2 and 3); lane 5, 3T3-L1 pCMVneo clone 1. All cDNAs were coamplified with GAPDH as an internal control. Bands of comparable intensity, obtained by the GAPDH sequence-specific primers, suggest comparable amplification of all samples. (C) 3T3-L1, 3T3-L1-HMGI(Y)as, 3T3-L1-HMGI(Y)s, and 3T3-L1 pCMVneo cell clones were treated with differentiating agents. Nuclear proteins were extracted and separated (20 µg/lane) by SDS-15% PAGE and transferred to polyvinylidene difluoride membranes. Western blots were incubated first with antibodies specific for the HMGI(Y) protein and then with horseradish peroxidase-conjugated secondary antibodies; the immunocomplexes were detected by enhanced chemiluminescence. As a control for equal loading, the blotted proteins were stained with Ponceau Red. The same Western blots were incubated with antibodies to the ubiquitous $gamma$ -tubulin protein. Sources of proteins were the following: lane 1, PC MPSV cells (positive control); lane 2, 3T3-L1 cells; lanes 3 and 4, 3T3-L1-HMGI(Y)as cells (clones 1 and 2); lane 5, 3T3-L1 pCMVneo clone 1; lanes 6, 7, and 8, 3T3-L1-HMGI(Y)s cells (clones 1, 2, and 3).

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FIG. 3. (A) Inhibition of adipocytic differentiation induced by blockage of HMGI(Y) synthesis. Adipogenic differentiation of normal and pCMVneo- or pCMV-HMGI(Y)as-transfected 3T3-L1 cells is shown. Cell clones were cultured in the presence of standard differentiation induction medium containing 0.5 mM 1-methyl-3-isobutylxanthine, 1 mM dexamethasone, 5 µg of insulin/ml, and 10% fetal bovine serum. After 8 days of differentiation, cells were observed by light microscopy. Magnification, ×400. This experiment is representative of five independent assays. (B) mRNA levels of aP2 and leptin were determined by RT-PCR, gel electrophoresis, and Southern blot hybridization. For details, see Materials and Methods. The cDNAs were coamplified with GAPDH, as an internal control. No bands are seen in non-reverse-transcribed RNAs, thus excluding DNA contamination (data not shown). RNAs were extracted from these cells at days 0, 4, and 7 of differentiation, as indicated.

Since differentiation of 3T3-L1 cells requires arrest of growth in G₁, we investigated whether HMGI(Y) affected the 3T3-L1growth rate. The 3T3-L1-HMGI(Y)as cells had a much shorter doublingtime (15.4 h) and an increased growth rate compared with the parentalcells (doubling time, 22.8 h) (Fig. 4A). Conversely, the 3T3-L1-HMGI(Y)scells showed an opposite phenotype, with an increased doublingtime (29.4 h) and a reduced growth rate (Fig. 4A). For 3T3-L1cells undergoing adipocytic differentiation, there is a G₁/G₀arrest at confluence, followed by a phase of clonal expansioninitiated by the differentiating agents (35), and a subsequentarrest about 2 days later. The G₁/G₀ arrest was observed in parentaland 3T3-L1-HMGI(Y)s cells but not in 3T3-L1-HMGI(Y)as clones (Fig.4B). We also evaluated the effect of the HMGI(Y) protein on cellgrowth by performing a colony-forming assay. Exponentially growing3T3-L1 cells were transfected with the HMGI(Y)as and HMGI(Y)sconstructs and with the empty vector, selected with G418, andcounted. Suppression of HMGI(Y) protein synthesis determined aremarkable increase in the number of colonies (387 colonies, comparedto 46 with the empty vector), whereas its overexpression determineda reduction in the number of colonies (12 colonies). Therefore,these results indicate that HMGI(Y) exerts a negative effect onthe growth rate of 3T3-L1 cells.

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FIG. 4. (A) Cells were grown as described in Materials and Methods and counted daily. (B) Cells were grown until confluence and then induced to differentiate as described in Materials and Methods. Cell counts started 1 day after the addition of the differentiation cocktail, as indicated, and were performed daily. For each type of experiment, one representative clone is shown; the results were confirmed on two additional clones. The data reported are the average results of two independent experiments.

HMGI(Y) physically interacts with C/EBP proteins. Transcriptional regulation of adipocyte differentiation requires the concerted activity of several transcription factors thatcontrol growth arrest and the coordinated expression of adipocyte-specificgenes. Among these transcription factors, C/EBP proteins playa critical role in the development of the adipocyte differentiationprogram. Indeed, the levels of the C/EBP proteins increase duringadipocyte differentiation. The increase of C/EBP $beta$ and C/EBP $delta$ occursearly during differentiation and is followed by the increase ofC/EBP $alpha$ , which ultimately controls the expression of several genes,among which are the genes for aP2 and leptin (26). Our dataindicated that HMGI(Y) proteins are also required for differentiationof 3T3-L1 preadipocytes. These observations suggested that HMGI(Y)might influence adipocytic differentiation through interactionswith the C/EBP transcription factors. To test this hypothesis,3T3-L1 cells were synchronously differentiated into adipocytesby hormonal treatment. Cells were harvested at time zero and atvarious times during differentiation, and the interaction betweenC/EBP $beta$ and HMGI(Y) was examined by coimmunoprecipitation experiments.Protein extracts were immunoprecipitated with anti-C/EBP $beta$ antiseraand immunoblotted with anti-HMGI(Y) antibodies (Fig. 5A, upperpanel). Interaction between C/EBP $beta$ and HMGI(Y) was detected attime zero; it increased at 6 h and remained stable until day 6of differentiation. This interaction was not detected when a preimmuneserum was used for lysate extracts of 6 h (Fig. 5A). In agreementwith previous observations, C/EBP $beta$ levels increased during earlydifferentiation of 3T3-L1 cells (Fig. 5A, lower panel). We alsodetected binding of HMGI(Y) and the other two C/EBP proteins (notshown); these interactions occurred with different kinetics.

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FIG. 5. (A) Interaction between C/EBP $beta$ and HMGI(Y). Cell lysates were prepared from 3T3-L1 cells at the indicated times as described in Materials and Methods. Proteins were immunoprecipitated with antibodies directed against the protein C/EBP $beta$ (Santa Cruz Biotechnology), as indicated. Immunoprecipitated (I.P.) proteins were immunoblotted with anti-HMGI(Y). Levels of C/EBP $beta$ during differentiation are shown. IgG, immunoglobulin G. (B) Wild-type C/EBP $beta$ protein was in vitro translated as described in Materials and Methods. Rabbit reticulocyte extracts were mixed with GST-HMG-Y recombinant protein for binding assays. Binding reaction products were washed, and proteins were separated on a polyacrylamide gel. Filters were probed with the anti-C/EBP $beta$ antibody (Santa Cruz Biotechnology). (C) C/EBP $beta$ and HMGI(Y) interaction in 293 cells. 293 cells were transfected with the indicated expression plasmids as described in Materials and Methods. Cell lysates were prepared, and equal amounts of proteins were immunoprecipitated with the indicated antibodies. In the top two panels, lane 1 shows a control immunoprecipitation. In lanes 2 and 3, the indicated cell lysates were immunoprecipitated either with the anti-C/EBP $beta$ antibody (upper panel) or with the anti-HMGI(Y) antibody. The immunocomplexes were immunoblotted with the reciprocal antibodies, as indicated. In the bottom two panels, Western blot analysis shows the amounts of C/EBP $beta$ and HMGI(Y) for each lysate used in the top two panels.

To verify these interactions, we carried out in vitro and in vivo binding studies with C/EBP $beta$ and HMGI(Y). C/EBP $beta$ was synthesizedin vitro by using rabbit reticulocyte lysates, and HMGI(Y) wasproduced as a GST fusion protein and bound to glutathione-agarosebeads (GST-Y). A pull-down assay was performed by incubating thetwo proteins. GST-bound proteins were immunoblotted on Immobilon-Pand detected with anti-C/EBP $beta$ antibodies. As shown in Fig. 5B,GST-Y, but not GST, was able to coprecipitate with C/EBP $beta$ . Forthe in vivo binding assays, the plasmids encoding C/EBP $beta$ and HMGI(Y)were transiently transfected in 293 cells. The cDNA encoding C/EBP $beta$ was expressed in the 293 cells alone and with HA-HMGI(Y). Cellextracts were immunoprecipitated with anti-C/EBP $beta$ or with anti-HMGI(Y)antibodies and immunoblotted with the reciprocal antisera. Coexpressionof C-EBP $beta$ and HMGI(Y) resulted in reciprocal coimmunoprecipitationof the two proteins (Fig. 5C). Analogous results were obtainedby using C/EBP $alpha$ and C/EBP $delta$ , which also bound to HMGI(Y) in vivoand in vitro (data notshown).

Mapping of the HMGI(Y) region responsible for binding to C/EBP $beta$ . To map the HMGI(Y) region required for binding to C/EBP $beta$ , we generated a series of progressive deletions of the HMGI(Y) genein an area corresponding to the carboxy-terminal region of itsproduct (Fig. 6A). The resulting cDNAs were tagged with the influenzavirus HA epitope and cloned into the pCEFL expression vector.Immunoblotting analysis showed that approximately equal amountsof wild-type and mutant proteins were produced. These mutantswere tested for their interaction in vivo with C/EBP $beta$ in coimmunoprecipitationexperiments. Each HMGI(Y) plasmid was transfected in 293 cellstogether with a C/EBP $beta$ -expressing vector. Thirty-six hours aftertransfection, cells were harvested and protein extracts were immunoprecipitatedwith anti-C/EBP $beta$ antibodies. As shown in Fig. 6B, deletion ofthe carboxy-terminal tail and of the third basic repeat did notimpair the binding of the HMGI(Y) protein to C/EBP $beta$ [compare wild-typeHMGI(Y) with mutant 1-63]. Conversely, removal of the region betweenthe middle and the last basic repeat (amino acids 54 to 63) andof the second repeat is detrimental to the interaction of HMGI(Y)with C/EBP $beta$ [compare wild-type HMGI(Y) with mutants 1-53 and 1-43].These results demonstrate that the carboxy-terminal tail and thethird basic repeat are not essential for this interaction, whereasthe region between the second and third repeats is required forthe binding of HMGI(Y) and C/EBP $beta$ .

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FIG. 6. The region between the second and the third AT hook is required for HMGI(Y)-C/EBP $beta$ interaction. (A) Schematic diagram of plasmids expressing HA-tagged wild-type HMGI(Y), showing the 1- 63, 1-53, and 1-43 deletion mutant proteins. The HA epitope tag, AT hooks (+), and C-terminal (----) domains are also indicated. (B) 293 cells were transiently cotransfected with C/EBP $beta$ and the indicated HMGI(Y) mutant plasmids. Equal amounts of cell lysates (2 mg) were immunoprecipitated with anti-C/EBP $beta$ antibodies, and the immunocomplexes were probed with either anti-C/EBP $beta$ (upper panel) or anti-HA antibodies (lower panel). Aliquots of the same lysates (50 µg) were probed with anti-HA antibodies to evaluate the comparable expression of the transfected plasmids.

HMGI(Y) cooperates with C/EBP in the regulation of the obese gene promoter, a C/EBP-regulated gene. The foregoing results suggested that C/EBP $beta$ cooperates with HMGI(Y) in the activation and/or repression of adipocyte-specificgene promoters. We focused on the promoter of the leptin protein,encoded by the obese gene, since its expression during adipocyticinduction seems to depend on HMGI(Y) synthesis. We first usedthe obese (ob) minimal promoter ( $-$ 161), which contains C/EBP motifsand which is a natural target of C/EBP transcription factors (20,28). A plasmid containing the ob minimal promoter fused to theluciferase reporter gene ( $-$ 161 ob-luc) was transfected in 293cells with or without C/EBP $beta$ . As shown in Fig. 7A, C/EBP $beta$ activatedluciferase transcription. When C/EBP $beta$ was cotransfected with HMGI(Y),activation of the ob promoter was significantly potentiated. Conversely,no activation was observed in the presence of HMGI(Y) alone orwhen the m52-ob-luc promoter, which is mutated in the C/EBP-bindingsite, was used for the cooperativity assay. Analogous resultswere obtained when we used the ob-luc-762 long promoter (datanot shown). As a further control for the specificity of the stimulatoryeffect of HMGI(Y) on C/EBP-mediated transactivating activity,we used another reporter vector, RSV-luc. This vector containsa promoter which has a low basal activity in 293 cells and isinsensitive to C/EBP. As shown in Fig. 7B, neither C/EBP $beta$ or HMGI(Y)alone nor the combination of the two proteins was able to significantlystimulate this promoter. Moreover, we have demonstrated that HMGI(Y)is also able to cooperate with C/EBP $alpha$ in the transactivation ofthe leptin promoter (data not shown).

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FIG. 7. (A) Leptin transactivation by C/EBP $beta$ and cooperation with HMGI(Y). Histograms show the luciferase activities of extracts from 293 cells cotransfected with the p( $-$ 161)ob-luc reporter and the indicated C/EBP $beta$ and HMGI(Y) plasmids. The mutant m52 reporter plasmid was used as a negative control. (B) Histograms showing the luciferase activities of extracts from 293 cells cotransfected with the RSV-luc reporter and the C/EBP $beta$ and HMGI(Y) plasmids. The relative activities were calculated by dividing the normalized activities by the activity of the m52 and RSV-luc constructs, which has been considered equal to 1. The data represent the average of results of three independent experiments, performed in duplicate, with standard deviations. (C) After transfection, cell lysates were divided into two aliquots. One of these aliquots was used for transactivation assays, and the other was used for Western blot analysis as a control of protein expression. Protein extracts were separated by SDS-PAGE, transferred to Immobilon-P, and immunoblotted with the indicated antibodies.

We then asked whether physical interaction between HMGI(Y) and C/EBP $beta$ was important for the potentiation of leptin transcription.We tested the HMGI(Y) deletion mutant 1-63, which is still ableto bind C/EBP $beta$ , and the mutants 1-53 and 1-43 (Fig. 7A), whichare defective in binding C/EBP $beta$ , for their ability to activatethe ob-luc promoter in the presence of C/EBP $beta$ . As shown in Fig.7A, mutant 1-63 behaved like wild-type HMGI(Y) in the C/EBP $beta$ -mediatedtransactivation assay. When mutant 1-53 was used, there was asignificant (more than 50%) reduction of activity in the cooperativityassay. When we used mutant 1-43, the effect was more dramatic,i.e., a sixfold loss of activity. These results suggest that deletionof residues 54 to 63, which are important for interaction betweenHMGI(Y) and C/EBP $beta$ , partially impairs their functional cooperation.The more dramatic phenotype observed with the 1-43 mutant, whichalso lacks the second basic repeat of HMGI(Y), suggests that theHMGI(Y) 43-to-53 region mediates the activation of the leptinpromoter independently from its ability to bind C/EBP. Westernblot analysis showed that the transfected cells expressed adequatelevels of the C/EBP $beta$ and HMGI(Y) proteins (Fig. 7C).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Adipocytic differentiation requires HMGI(Y). HMGI(Y) and HMGI-C proteins are important architectural transcription factors (19), and a growing body of evidence suggeststhat they are involved in adipocytic differentiation (2, 34,40, 49). We have investigated the role of HMGI(Y) proteinsin adipogenesis using 3T3-L1 preadipocytic cells as a model system.Northern and Western blot analyses demonstrated induction of theHMGI(Y) gene and protein when 3T3-L1 cells were induced to differentiateinto adipocytes. HMGI(Y) expression is detectable at very lowlevels in growing, undifferentiated 3T3-L1 cells and increasesduring differentiation. These observations suggested that an increasein HMGI(Y) levels is necessary for 3T3-L1 differentiation. Indeed,suppression of HMGI(Y) protein synthesis through antisense methodologyprevented terminal adipocytic differentiation. Not only did thesecells not show the typical fat-laden phenotype, but they alsolacked the expression of two adipocytic markers, aP2 and leptin.On the other hand, forced expression of the HMGI(Y) gene resultedin inhibition of growth, but it was not able to induce differentiation.These data demonstrated that the wild-type HMGI(Y) protein isrequired, but not sufficient, for 3T3-L1 cells to differentiateinto adipocytes. Three members of the C/EBP family of transcriptionfactors (C/EBP $alpha$ , - $beta$ , and - $delta$ ) have been implicated in the inductionof adipocyte differentiation. In particular, overexpression ofC/EBP $alpha$ is sufficient to arrest growth and to start the adipocytedifferentiation program in preadipocytic cell lines (26). Recentdata obtained in our laboratory indicate that its forced expressionin the 3T3-L1 HMGI(Y)as cells is not able to revert their phenotype,i.e., the block of growth arrest and adipocytic differentiation(data not shown). These data indicate that HMGI(Y) is indeed necessaryfor C/EBP $alpha$ to induce its biological effects. This hypothesis isalso supported by results of other experiments. The promotersof several adipocyte-specific genes contain C/EBP regulatory bindingsites. For instance, C/EBP $alpha$ was shown to bind and transactivatethe aP2 promoter. Furthermore, the leptin promoter contains atleast one functional C/EBP binding site: disruption of this consensussequence by site-directed mutagenesis causes a remarkable decreasein promoter activity (20, 28). Based on these observations,we argued that HMGI(Y) modulates the transcriptional activityof the C/EBPs. This hypothesis was confirmed by the finding thatHMGI(Y) physically interacts with C/EBP transcriptionfactors.

HMGI(Y) proteins suppress 3T3-L1 cell proliferation. In 3T3-L1 cells undergoing adipocyte differentiation, there is a G₁/G₀ arrest at confluence, followed by a phase of clonalexpansion initiated by the differentiating agents (26) and asubsequent arrest about 2 days later. We show that suppressionof HMGI(Y) expression causes a blockage in the differentiationassociated with an increased growth rate in 3T3-L1 cells. Furthermore,treatment of HMGI(Y) antisense-expressing cells with differentiatingagents failed to induce the cell cycle arrest that precedes differentiation.Therefore, we suggest that HMGI(Y) plays a critical role in adipocyticcell growth. The levels of HMGI(Y) do not correlate with the cellcycle status of the cells during induction of differentiation,being highest in the phase of mitotic clonal expansion (6 h andday 1) and reduced in growth-arrested, differentiating cells (days0 and 4). This paradox could be explained by the fact that HMGI(Y)is an accessory protein, with multiple functions, for a wide rangeof transcription factors. Its effect could enhance growth arrestor proliferation depending on the presence of different transcriptionfactors.

Our data indicate that the role of HMGI(Y) in the control of adipocytic cell growth counteracts that of HMGI-C. In fact, whileoverexpression of HMGI(Y) negatively regulates adipocytic cellgrowth, HMGI-C expression seems to be necessary for physiologicalproliferation of adipocytes. Indeed, HMGI-C knockout mice displaya pygmy phenotype with a remarkable reduction of the adipose tissue(49), and the suppression of the HMGI-C synthesis blocks proliferationof the 3T3-L1 cells (S. Battista et al., unpublished data). Wesuggest that the growth of adipocytic cells results from the balancebetween levels of HMGI-C and HMGI(Y). From the data presentedhere, the role of HMGI(Y) seems to be pleiotropic, depending onthe cellular context. HMGI(Y) proteins often have been associatedwith cell proliferation: in fact, HMGI(Y) has been found overexpressedin several experimental and human malignant tumors (1, 3,8, 9, 16, 17, 36), and overexpression of HMGI(Y) causestransformation of Burkitt's lymphoma cells (43). Consistentwith the hypothesis that the different cellular context may accountfor the different effects of overexpression of the HMGI(Y) gene,we have also recently demonstrated that overexpression of HMGI(Y)impairs the growth of normal PC Cl 3 rat thyroid cells by inducingapoptosis (M. Fedele et al., unpublished data). In our opinion,this hypothesis seems to be likely, since several genes involvedin the control of cell proliferation can induce different biologicaleffects, such as cell growth, differentiation, and apoptosis,depending on the cellularcontext.

The involvement of HMGI(Y) and HMGI-C in adipocytic cell growth has interesting implications for the pathogenesis of somehuman tumors. Indeed, the HMGI-C and HMGI(Y) genes are involvedin chromosome translocations occurring in benign mesenchymal tumors,including lipomas (2, 12, 34, 40, 45). Consequent tothe translocation, HMGI proteins fuse to heterologous genes, orthey simply lose the carboxy-terminal domain and retain only theDNA-binding domain. Consistently, the expression of a truncatedform of the protein (containing only DNA-binding domains) resultsin enhanced proliferation of 3T3-L1 cells (G. M. Pierantoni etal., unpublisheddata).

HMGI(Y) proteins physically interact with C/EBP $beta$ and modulate C/EBP-mediated transcription. C/EBPs play a pivotal role in adipogenesis (6, 37). Here we demonstrate that HMGI(Y) binds to C/EBP $beta$ in 3T3-L1 cellsand in 293 cells by reciprocal coimmunoprecipitation. We alsoshow that a GST-HMGI(Y) fusion protein binds C/EBP in a typicalpull-down assay. Furthermore, we demonstrate that this bindingrequires the region between amino acids 53 and 63 of HMGI(Y).By binding to C/EBPs, HMGI(Y) may functionally cooperate withthese proteins to activate and/or repress different promoters.Preliminary results obtained by using band shift analysis witha C/EBP-specific oligonucleotide show that high-molecular-weightcomplexes are formed at different times during 3T3-L1 differentiation(G. M. Pierantoni and R. M. Melillo, personal communication):HMGI(Y) may be involved in the assembly of higher-order complexesthat are essential for both arrest of growth and the expressionof the differentiated phenotype of adipocyte precursors. Consistentwith the idea that HMGI(Y) serves as a general cofactor of adipocyte-specifictranscription, we observed that HMGI(Y) expression modulates thetranscription of a gene whose levels are regulated during adipocytedifferentiation: the obese gene coding for leptin (48). BothC/EBP $alpha$ and C/EBP $beta$ bind to the C/EBP consensus site on the leptinpromoter and are able to activate transcription of the obese gene(28). Here we show that HMGI(Y) functions as a specific cofactorfor C/EBP $beta$ . Indeed, we demonstrate that C/EBP $beta$ -mediated activationof the leptin promoter was strongly potentiated by the presenceof the HMGI(Y) protein. The same results were obtained with theC/EBP $alpha$ transcription factor, suggesting that HMGI(Y) is an accessoryfactor for this family of proteins. This is consistent with theobservation that HMGI(Y) is also able to bind to C/EBP $alpha$ and - $delta$ (data not shown). Analysis of the obese minimal promoter sequencefailed to identify putative HMGI(Y)-DNA binding sites, which arerepresented by tracts of adenines and thymines arranged on thesame face of the DNA helix. Furthermore, electrophoretic mobilityshift analysis performed in vitro with purified recombinant HMGI(Y)and the ob minimal promoter showed no high-affinity HMGI(Y) DNA-bindingsites (Pierantoni and Melillo, personal communication). Theseobservations, together with the ability of HMGI(Y) to bind C/EBPin solution in the absence of DNA, argue against the presenceof HMGI(Y) in C/EBP-DNA complexes: it is possible that HMGI(Y)facilitates the binding of C/EBP to DNA by transiently associatingwith C/EBP.

We also mapped the domain of HMGI(Y) that is required for its functional cooperation with C/EBP $beta$ . Deletion of the region betweenthe third and the second AT hook impaired the ability of HMGI(Y)to cooperate with C/EBP $beta$ . Interestingly, this region is also requiredfor efficient HMGI(Y) and C/EBP $beta$ binding, confirming that physicalinteraction between the two factors contributes to efficient functionalcooperation. We show that a further deletion, which abrogatesthe second AT hook, completely abolishes the cooperation of HMGI(Y)and C/EBP $beta$ . Consequently, the second AT hook also plays a rolein the activation of the ob promoter. The cooperation betweenHMGI(Y) and C/EBP in the transactivation of the leptin promotercould be explained by several mechanisms, which are not mutuallyexclusive. One possibility is that the binding of HMGI(Y) to C/EBPcould enhance the affinity of C/EBP for its target DNA. Such amechanism has been demonstrated for other transcription factors,such as NF- $kappa$ B (47). Alternatively, HMGI(Y) could recruit oneor more components of the basal transcriptional machinery to theprotein-DNA complexes, thus enhancing transcription. Whateverthe mechanism, protein-protein interaction between HMGI(Y) andC/EBP $beta$ might favor the activity of the C/EBP transcriptional complex.However, our data seem also to indicate that there is only a partialcontribution of this interaction to the cooperation between HMGI(Y)and C/EBP $beta$ in transactivating the leptin promoter. This suggeststhat other functions, dependent on HMGI(Y) residues 43 to 53,are important for thiscooperation.

Furthermore, preliminary data obtained in our laboratory show that HMGI(Y) and C/EBP $beta$ negatively regulate the promoter ofthe Id1 gene, whose expression is down-regulated during adipogenesisand correlates with growth arrest that precedes differentiation(30, 31).

Conclusions. The data presented here show that HMGI(Y) exerts a negative effect on the proliferation of adipocyte precursors and a positiveeffect on differentiation. This dual role is consistent with thefinding that HMGI proteins may positively and negatively affectgene expression. We also demonstrate that the HMGI(Y) proteinphysically interacts with C/EBP proteins and that it functionallycooperates in the transcriptional activity mediated by these proteins,whose function is required to trigger the expression of adipocyte-specificgenes.

	ACKNOWLEDGMENTS

This study was supported by the Associazione Italiana per la Ricerca sul Cancro (AIRC), the Progetto Finalizzato Biotecnologieof Consiglio Nazionale delle Ricerche. G.M.P. and A.S. are supportedby a Fondazione Italiana per la Ricerca sul Cancro (FIRC)fellowship.

We are grateful to Jean Gilder for revising and editing the text. We are indebted to D. Thanos for the HMGI(Y) deletion mutantsand to M. Reitman for the p( $-$ 762)ob-luc, p( $-$ 161)ob-luc, and m52plasmids. We also thank Fernando Sferratore for excellent technicalassistance.

	FOOTNOTES

^* Corresponding author. Mailing address: Dipartimento di Biologia e Patologia Cellulare e Molecolare, Facoltà di Medicina eChirurgia, Via Pansini, 5, 80131 Naples, Italy. Phone: 39 0817463056. Fax: 39 081 7463037 or 7701016. E-mail: afusco{at}napoli.com.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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36. Tamimi, Y., H. G. van der Poel, M. M. Denym, R. Umbas, H. F. M. Karthaus, F. M. J. Debruyne, and J. A. Schalken. 1993. Increased expression of high mobility group protein I(Y) in high-grade prostate cancer determined by in situ hybridization. Cancer Res. 53:5512-5516[Abstract/Free Full Text].

37. Tanaka, T., N. Yoshida, T. Kishimoto, and S. Akira. 1997. Defective adipocyte differentiation in mice lacking the C/EBP $beta$ and/or C/EBP $delta$ gene. EMBO J. 24:7432-7443[CrossRef].

38. Thanos, D., and T. Maniatis. 1992. The high mobility group protein HMG I(Y) is required for NF- $kappa$ B dependent virus induction of the human IFN- $beta$ gene. Cell 71:777-789[CrossRef][Medline].

39. Thanos, D., and T. Maniatis. 1995. Virus induction of human IFN beta gene expression requires the assembly of an enhanceosome. Cell 83:1091-1100[CrossRef][Medline].

40. Tkachenko, A., H. R. Ashar, A. M. Meloni, A. A. Sandberg, and K. K. Chada. 1997. Misexpression of disrupted HMGI architectural factors activates alternative pathways of tumorigenesis. Cancer Res. 57:2276-2280[Abstract/Free Full Text].

41. Tontonoz, P., E. Hu, and B. M. Spiegelman. 1994. Stimulation of adipogenesis in fibroblasts by PPAR $gamma$ , a lipid-activated transcription factor. Cell 79:1147-1156[CrossRef][Medline].

42. Umek, R. M., A. D. Friedman, and S. L. McKnight. 1991. CCAAT/enhancer-binding protein: a component of a differentiation switch. Science 251:288-292[Abstract/Free Full Text].

43. Wood, L. J., M. Mukherjee, C. E. Dolde, Y. Xu, J. F. Maher, T. E. Bunton, J. B. Williams, and L. M. Resar. 2000. HMGI/Y, a new c-Myc target gene and potential oncogene. Mol. Cell. Biol. 20:5490-5502[Abstract/Free Full Text].

44. Wu, Z., N. L. R. Bucher, and S. R. Farmer. 1996. Induction of peroxisomeproliferator-activated receptor $gamma$ during the conversion of 3T3 fibroblasts into adipocytes is mediated by C/EBP $beta$ , C/EBP $delta$ , and glucocorticoids. Mol. Cell. Biol. 16:4128-4136[Abstract].

45. Xiao, S., M. L. Lux, R. Reeves, T. J. Hudson, and J. A. Fletcher. 1997. HMGI(Y) activation by chromosome 6p21 rearrangements in multilineage mesenchymal cells from pulmonary hamartoma. Am. J. Pathol. 150:901-910[Abstract].

46. Yeh, W.-C., Z. Cao, M. Classon, and S. L. McKnight. 1995. Cascade of terminal adipocyte differentiation by three members of the C/EBP family of leucine zipper proteins. Genes Dev. 9:168-181[Abstract/Free Full Text].

47. Zhang, X. M., and G. L. Verdine. 1999. A small region in HMGI(Y) is critical for cooperation with NF- $kappa$ B on DNA. J. Biol. Chem. 274:20235-20243[Abstract/Free Full Text].

48. Zhang, Y., R. Proenca, M. Maffei, M. Barone, L. Leopold, and J. L. Friedman. 1994. Positional cloning of the mouse obese gene and its human homologue. Nature 372:425-432[CrossRef][Medline].

49. Zhou, X., K. F. Benson, H. R. Ashar, and K. K. Chada. 1995. Mutation responsible for the mouse pygmy phenotype in the developmentally regulated factor HMGI-C. Nature 376:771-774[CrossRef][Medline].

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