Stat3beta  Inhibits gamma -Globin Gene Expression in Erythroid Cells

doi:10.1074/jbc.M106556200

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Stat3 $beta$ Inhibits $gamma$ -Globin Gene Expression in Erythroid Cells^*

Heather A. Foley, Solomon F. Ofori-Acquah, Akihiko Yoshimura^§, Stuart Critz, B. Surendra Baliga^¶, and Betty S. Pace^¶

From the Department of Cell Biology and Neuroscience, University of South Alabama, Mobile, Alabama 36688, the ^§ Department of Molecular and Cellular Immunology, Kyushu University, Fukuoka, Japan, and the ^¶ Department of Pediatrics, University of South Alabama, Mobile, Alabama 36606

Received for publication, July 12, 2001, and in revised form, January 30, 2002

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

We demonstrated previously $gamma$ -globin gene inhibition in K562 cells and primary erythroid progenitors treated with interleukin-6.Although several cis-acting elements have been identified in theglobin promoters, the precise mechanism for cytokine-mediatedglobin gene regulation remains to be elucidated. In this reportwe demonstrate inhibitors of Stat3 phosphorylation abrogate interleukin-6-mediated $gamma$ gene silencing in erythroid cells. DNA-protein binding studiesestablished Stat3 interaction in the 5'-untranslated $gamma$ -globinpromoter region. Furthermore, co-transfection experiments withStat3 $beta$ demonstrate $gamma$ promoter inhibition in a concentration-dependentmanner, which was significantly reversed when the cognate Stat3-bindingsite in the 5'-untranslated region was mutated. These studiesestablish a novel mechanism for $gamma$ gene silencing through the STATsignal transductionpathway.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Signal transducers and activators of transcription (STATs)¹ play an essential role in regulating gene expression via a varietyof pathways involving cytokines, growth factors, and other extracellularstimulants. Protein tyrosine kinases of the Janus kinase (JAK)family activate STAT proteins upon binding of cytokines to theircognate receptors (1, 2). The JAK-STAT pathway mediatesthe effect of several cytokines (3-5) including interleukin 6(IL-6), which was previously demonstrated to inhibit $gamma$ gene expression(6) and to most likely exert its negative effect at the levelof the bi-potential progenitor cell. Although several cis-actingelements have been identified in the globin gene promoters (7,8), the precise mechanism for cytokine-mediated globin generegulation during development remains to beclarified.

Receptor-bound IL-6 stimulates glycoprotein 130 homodimerization and ligand-dependent JAK2 activation (9, 10). ActivatedJAK2 phosphorylates the cytoplasmic domain of glycoprotein 130creating docking sites for dimerization of Stat1 and Stat3. Thephosphorylated dimer molecules translocate into the nucleus andbind IL-6-response elements in target promoters. Stat3 $beta$ is a naturallyoccurring splice variant of Stat3 $alpha$ with a deletion of the carboxyl-terminal55 amino acid residues including Ser-727, which is important forefficient transcriptional activation (11-14). Stat3 $beta$ efficientlybinds to the palindromic IL-6-response element as a homodimerbut lacks transcriptional activity alone and is generally considereda dominant negative regulator (15). However, Schaefer et al.(16) demonstrated $alpha$ ₂-macroglobulin gene activation via Stat3 $beta$ -c-Juninteractions. Likewise, murine Stat3 $beta$ has been shown to activateselected promoters in a cell type-specific manner (16).

In this report we demonstrate abrogation of the IL-6-mediated $gamma$ gene repression in K562 cells pretreated with the JAK2 andStat3/Stat5 inhibitors AG490 and piceatannol (PIC), respectively.Moreover, PIC reversed IL-6-mediated $gamma$ gene silencing in primaryerythroid cells grown from adult and fetal stage progenitors.Western blot analysis confirmed that IL-6 preferentially activatedStat3 $beta$ in K562 cells. Subsequent experiments completed in a geneticreporter system demonstrated a concentration-dependent Stat3 $beta$ -mediated $gamma$ gene silencing. Targeted mutagenesis of the cognate Stat3-bindingsite in the $gamma$ promoter reversed the negative effects of Stat3 $beta$ on $gamma$ gene expression. Our studies establish a novel role for STATproteins in globin gene regulation and a mechanism whereby Stat3inhibits $gamma$ -globin geneactivity.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Cell Lines-- K562 erythroleukemia cells were cultured under the following conditions: RPMI 1640 containing 10% fetal bovine serum, penicillin(100 units/ml), and streptomycin (0.1 mg/ml) in a humidified incubatorat 37 °C, 5% CO₂. Cells were treated for 48 h with either IL-6(100 ng/ml) or sodium butyrate (NaB, 2 mM) (Sigma) alone or followingpretreatment with the inhibitors PIC (10 µM) for 30 min, AG490(25 µM) for 16 h, or UO126 (10 µM) for 1 h. All inhibitors werepurchased from Calbiochem.

Burst-forming Unit-Erythroid (BFU-E) Colony Growth-- Peripheral and umbilical cord blood samples were obtained from normal individuals after informed consent was obtained in accordancewith the University of South Alabama Institutional Review Boardguidelines. Mononuclear cells were isolated by density gradientcentrifugation (Histopaque-1077, Sigma) and pretreated for 30min with PIC (10 µM) where indicated. Erythroid progenitors werecultured in methylcellulose as published previously by the authors(17), and NaB (1 mM) or IL-6 (100 ng/ml) was added on day 0of culture. BFU-E colonies were counted and harvested on day 14,and fetal hemoglobin (HbF) was measured as a percent of totalhemoglobin, normalized to total protein, by alkaline denaturationas published previously (17, 18).

RNA Isolation and RNase Protection Assay-- Total RNA from BFU-E colonies and K562 cells was isolated using RNA Stat-60 (Tel-Test, Friendswood, TX) according to the manufacturer'sinstructions. RNase protection assay (RPA) was performed withprobes designed to yield different size protected fragments for $gamma$ -globin (170-bp) and glyceraldehyde-3-phosphate dehydrogenase(GAPD, 354-bp) mRNA. The level of mRNA transcripts was quantitatedby PhosphorImager analysis (GS-250, Bio-Rad) as described previously(19). $gamma$ -Globin mRNA was normalized to that of GAPD.

Preparation of Cytosolic Protein Extracts-- K562 cells were lysed in 500 µl of ice-cold lysis buffer (75 mM NaCl, 50 mM NaF, 20 mM HEPES, 2.5 mM MgCl₂, 15 mM EGTA, 2mM EDTA, 1% Triton X-100, 0.1 mM Na₃PO₄, 0.5 mM dithiothreitol,4 µg of leupeptin, 200 µg of phenylmethylsulfonyl fluoride, pH7.4). Cellular debris was removed by centrifugation, and proteinconcentrations were determined with the Bradford assay (Bio-Rad).Aliquots of 25 µg were frozen at $-$ 70 °C until used to avoid theadverse effects of freeze-thaw cycles on proteinfunction.

Western Blot-- Cytosolic protein extracts (25 µg) were resolved by electrophoresis using 10% SDS-PAGE. Proteins were transferred to nitrocellulosemembranes and blocked with Tris-buffered saline containing 0.1%Tween 20 (TBS-T) and 5% dry milk for 1 h. The membranes were probedfor 12 h at 4 °C with total Stat3 antibody diluted 1:250 in TBS-Tor phopho-Stat3 antibody diluted 1:500 in TSB-T (Santa Cruz Biotechnology,Santa Cruz, CA). Both antibodies allow simultaneous measurementof Stat3 $alpha$ and Stat3 $beta$ levels. The membranes were washed and thenincubated for 1 h with anti-rabbit IgG-horseradish peroxidase(diluted 1:5000) in TBS-T for chemiluminescent detection. Thesame membranes were stripped and probed with an actin antibody(Santa Cruz Biotechnology) to control for any variations in theamount of protein loaded per well that may have occurred. Theintensity of each band was measured using imaging software (SigmaGel,Jandel Scientific, Chicago,IL).

Reporter Constructions-- Reporter plasmids were constructed with the pGL3-Basic luciferase plasmid (Promega, Madison, WI). The $gamma$ Luc plasmid was establishedby subcloning an AluI $gamma$ promoter fragment ( $-$ 299 to +36), froma plasmid containing a genomic clone, into the SmaI site of pGL3-Basic.HS2 $gamma$ Luc, a kind gift from Dr. Townes, contains the same promoterfragment as $gamma$ Luc downstream of the 1.9-kb hypersensitive site2 (HS2) enhancer from the $beta$ -globin locus control region. PlasmidDNA was extracted using the alkali lysis method and affinity purification(Qiagen Maxiprep System, Valencia,CA).

Site-directed Mutagenesis-- The A $gamma$ Stat3 site was mutated (mtA $gamma$ ) using an ExSite PCR-based Site-directed Mutagenesis Kit (Stratagene, La Jolla, CA). Briefly,a forward primer from nucleotide +9 to +30 in the $gamma$ promoter containingthe desired mutation 5'-TTTGAGAACGTCTGAGATTATC-3' and a 5'-phosphorylatedreverse primer from $-$ 14 to +8, 5'-GCGAGTGTGTGGAACTGCTGAA-3', weresynthesized for the PCR, using the wild-type HS2 $gamma$ Luc plasmid astemplate. The HS2 $gamma$ Luc plasmid was digested from the PCR productwith DpnI, followed by end polishing using Pfu DNA polymerase.The integrity of the PCR product was verified on an agarose gelfollowed by T₄ ligation and transformation into Epicurian Coli®XL1-Blue Supercompetent cells (Stratagene). The mutant carryingthe desired base substitution was confirmed by directsequencing.

Transient Transfections-- Two reporter plasmids $gamma$ Luc and HS2 $gamma$ Luc were analyzed in K562 cells. Each reporter plasmid (10 µg) was added to K562 cells(5 × 10⁶) and incubated at room temperature for 15 min followed by electroporationat 260 V and 975 microfarads (GenePulser, Bio-Rad). Transfectedcells were cultured as described above with the addition of IL-6(100 ng/ml) or NaB (2 mM) alone or in combination with signalingpathway inhibitors followed by chemical inductions. Cells wereharvested after 24 h and extracts prepared according to the manufacturer'sinstructions using a reporter lysis buffer (Promega). Proteinextracts (20 µl) were combined with 100 µl of enzyme reagent,and luciferase activity was measured (TD Luminometer, Promega).Total reporter gene activity was normalized to total protein.The relative luciferase activity was calculated as a ratio tothat of untreated controls. The pGL3 control vector was transfectedas a control with each experiment to monitor transfectionefficiency.

Three expression vectors Stat3 $alpha$ (pS3 $alpha$ ) and mutant Stat3 $alpha$ (pmS3 $alpha$ ) established in the base plasmid pDNA3.1 and Stat3 $beta$ (pS3 $beta$ )established in the pSG5 plasmid were tested. For trans-activatorexperiments 30 µg of plasmids was co-transfected with HS2 $gamma$ Luc(10 µg). Competition experiments were also completed by the simultaneousaddition of pmS3 $alpha$ and pS3 $beta$ or pS3 $alpha$ at a concentration of 15 µgeach to keep the total plasmid DNA constant at 30 µg. IL-6 (100ng/ml) exposure for 24 h was used to activate the Stat3 expressionvectors via phosphorylation. Experiments were also completed withpS3 $beta$ or pS3 $alpha$ alone at increasing concentrations from 10-50 µgor pS3 $beta$ held constant at 15 µg with increasing amounts of pS3 $alpha$ from 10 to 50 µg for competition studies. The pS3 $alpha$ and pmS3 $alpha$ vectorswere obtained from our collaborator Dr. Akihiko Yoshimura at theMedical Institute of Bioregulation, Japan. The pS3 $beta$ vector wasa kind gift from Dr. Richard Jove at the Moffitt Cancer Centerin Tampa,FL.

Electrophoretic Mobility Shift Assay (EMSA)-- K562 cells were induced with IL-6 for 48 h alone or after pretreatment with PIC or AG490 at the concentrations described above.Nuclear proteins were extracted as described by Andrews and Faller(20). The Biopolymer Core Facility of the University of SouthAlabama synthesized the oligonucleotides from the respective 5'-untranslatedregions for A $gamma$ -globin (A $gamma$ STAT3), $epsilon$ -globin ( $epsilon$ 5U), and $beta$ -globin( $beta$ 5U) that were used as EMSA probes (Fig. 3). The control Stat1and Stat3 oligonucleotides were purchased from Santa Cruz Biotechnology.The Stat1 consensus sequence is 5'-CATGTTATGCATATTCCTGTAAGTG-3';the Stat3 consensus sequence is 5'-GATCCTTCTGGGAATTCCTAGATC-3'.Underlined are the putative binding sites for the STAT transcriptionfactor. EMSAs were performed as follows. Double-stranded oligonucleotideswere end-labeled with [ $gamma$ -³²P]ATP using T₄ DNA kinase and purified on a G-25 spin column (AmershamBiosciences). Binding reactions were performed with 4 µg of nuclearprotein incubated with binding buffer (20% glycerol, 5 mM MgCl₂,2.5 mM EDTA, 250 mM NaCl, 50 mM Tris-HCl, pH 7.5) for 10 min atroom temperature, followed by incubation with radiolabeled probefor 20 min. For competition experiments 50-fold excess of coldcompetitor was incubated with the nuclear extract before additionof radiolabeled probes. For confirmatory antibody studies, theprobes were incubated with nuclear proteins for 15 min on iceand then STAT antibodies (2 µg) were added and incubated at 4°C overnight. All binding reactions were performed with 100-foldexcess of the nonspecific competitor poly(dI-dC) at a concentrationof 0.25 µg/ml. DNA-protein complexes were resolved on a 4% nondenaturingpolyacrylamide gel followed byautoradiography.

Statistical Analysis-- The data are reported as the means ± S.E. for at least four experiments. Statistical analysis of the raw data was performedby two tailed t tests. Student's t test was used to measure differencesin samples of two groups. Probability of less than 0.05 (p < 0.05)was consideredsignificant.

RESULTS

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Interleukin-6 Is Unique among Megakaryocytic Specific Cytokines in Its Ability to Inhibit $gamma$ -Globin-- We have demonstrated previously (6) that IL-6 reduces the steady-state level of $gamma$ -globin mRNA in BFU-E colonies and K562cells. This effect is evident in a concentration-dependent mannerand is concomitant with an increased level of glycoprotein IIbmRNA. To gain further insight into the role of other megakaryocyticspecific cytokines in $gamma$ gene regulation, we treated K562 cellswith thrombopoietin (25-300 ng/ml) or IL-11 (25-100 ng/ml) for72 h and found that neither cytokine had a significant effecton steady-state $gamma$ -globin mRNA levels. This suggests that IL-6is unique among the megakaryocytic specific cytokines in regulating $gamma$ globin.

Interleukin-6 Mediates $gamma$ Gene Inhibition via the JAK-STAT Signaling Pathway-- To determine the role of signaling proteins in the IL-6-mediated regulation of the $gamma$ -globin gene, we analyzed the effect ofspecific inhibitors of the JAK-STAT pathway. K562 cells were pretreatedwith AG490 or PIC prior to induction with IL-6. AG490 inhibitsthe ability of JAK2 to activate multiple downstream STAT proteins,whereas PIC specifically blocks activation of Stat3 and Stat5(21, 22). Steady-state $gamma$ -globin mRNA level remained unchangedin IL-6-induced K562 cells pretreated with either inhibitor suggestingthat the repressive effect of IL-6 was mediated through the JAK-STATpathway (Fig. 1, A and B). The effect of AG490 and PIC was similarto that observed with an anti-IL-6 antibody, which blocked theability of IL-6 to reduce $gamma$ -globin mRNA level by 50-60% (Fig.1B). The concentrations used for AG490 and PIC have been widelyapplied to inhibit effectively the JAK-STAT pathway (23). Toensure that the K562 cell line used in these experiments was responsiveto $gamma$ -globin gene activation, control experiments were performedwith NaB, which resulted in a 4.5-fold increase in $gamma$ -globin mRNAlevels. We conclude from these experiments that JAK2 and Stat3and/or Stat5 are necessary for the IL-6-mediated repression ofthe $gamma$ -globin gene.

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Fig. 1. Interleukin-6 inhibits $gamma$ -globin expression via the JAK-STAT pathway. K562 cells were treated with IL-6 alone or pretreated with anti-IL-6 antibody, AG490 or PIC. RPA was performed with a Hu $gamma$ probe yielding a 170-bp protected fragment and GAPD as an internal control. A, representative gel for the different conditions is shown. B, the quantitative data obtained from PhosphorImager analysis is depicted in the bar graph. Data are shown for uninduced (white bar), IL-6-treated (black bars), or sodium butyrate (gray bar)-treated K562 cells. The fold increased $gamma$ mRNA synthesis was calculated as a ratio to GAPD. The uninduced levels were normalized to 1. The data represent the mean ± S.E. Ud, untreated; Ab, IL-6 antibody; A, AG490; P, piceatannol. C, peripheral blood mononuclear cells were isolated and grown in methylcellulose culture for 14 days. Cellular RNA and proteins were isolated and analyzed by RPA and alkaline denaturation, respectively, as described under "Experimental Procedures." The effect of IL-6 or NaB on BFU-E colony growth (white bars), $gamma$ mRNA synthesis (black bars), and fetal hemoglobin (gray bars) levels for the different experimental conditions was analyzed. Untreated progenitor levels were normalized to 1. D, cord blood mononuclear cells were isolated and grown in methylcellulose culture as described under "Experimental Procedures." BFU-E colonies (white bars) and fetal hemoglobin levels (gray bars) are as shown for the different experimental conditions. Data represent the mean ± S.E.

To address the physiological relevance of this finding, we extended the studies with PIC to primary erythroid cells. Adultperipheral blood and umbilical cord blood mononuclear cells werecultured for 14 days in the presence of IL-6 alone or followingpretreatment with PIC. Cellular protein was isolated and HbF determinedby alkaline denaturation as a percent of total hemoglobin (18).In agreement with previous data from our laboratory (17, 18,24) and by others (25, 26), we observed an increase (1.5-fold)in BFU-E colony growth in adult peripheral blood cultures treatedwith IL-6 (Fig. 1C). However, steady-state $gamma$ -globin mRNA levelswere reduced by 6-fold (p < 0.05). The effect on mRNA synthesiswas reflected at the protein level by a significant reductionin HbF. In control experiments NaB increased $gamma$ mRNA and HbF levelsby 2.5- and 4.8-fold (p < 0.05), respectively. Prior treatmentof mononuclear cells with PIC on day 0 abrogated the ability ofIL-6 to repress HbF synthesis (data not shown). In contrast topromoting BFU-E colony growth from adult stage progenitors, IL-6restricted the expansion of BFU-E in cultures established withumbilical cord blood. Fig. 1D shows that IL-6 reduced BFU-E colonynumber by 5-fold and HbF by 6-fold in umbilical cord blood cultures.Interestingly, on this fetal-globin background there was concordanceof the IL-6 effect at the cellular and molecular level. It isworth noting that PIC abolished the effect of IL-6 on both cellproliferation and gene expression (Fig. 1D). The observation forgene control corroborates those observed in K562 cells and furtherimplicates STAT transcription factors as negative regulators of $gamma$ -globin gene expression. Our recent findings (24) from studyingmechanisms for $gamma$ -globin activation by short chain fatty acidsshow that $gamma$ -globin induction is associated with increased Stat5activation. It is therefore likely that the negative regulationof $gamma$ -globin reported here involves a variant ofStat3.

Interleukin-6 Induces Stat3 $beta$ Protein Synthesis in K562 Cells-- The potential for Stat3 involvement in $gamma$ -globin gene regulation was determined by analyzing the expression of Stat3 proteinsin IL-6-treated K562 cells. Cytosolic protein extracts were probedwith a polyclonal antibody that recognizes both Stat3 $alpha$ and thetruncated variant Stat3 $beta$ (Fig. 2A). Cells treated with IL-6 aloneshowed an insignificant increase in Stat3 $alpha$ , which was reducedto 50% below base-line values following pretreatment with PIC(Fig. 2B). By contrast the level of Stat3 $beta$ (80 kDa) increased5-fold in IL-6-treated K562 cells (p < 0.05). PIC inhibited Stat3 $beta$ induction by IL-6 and reduced endogenous Stat3 $beta$ levels to 80%below steady-state values (p < 0.05). AG490 had a less dramaticeffect on the levels of Stat3 induced by IL-6 generally. Thesedata demonstrate that IL-6 preferentially enhances Stat3 $beta$ expressionin K562 cells.

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Fig. 2. Interleukin-6 preferentially induces Stat3 $beta$ synthesis in K562 cells. A, schematic of wild-type Stat3 $alpha$ and the naturally occurring splice variant Stat3 $beta$ , with a deletion in the carboxyl-terminal trans-activation domain, is shown. The various DNA domains and the major sites of phosphorylation are as indicated. SH2, Src homology 2; Y, tyrosine residue 705; S, serine 727. B, Western blot analysis was performed on K562 cells to determine Stat3 $alpha$ and Stat3 $beta$ protein levels in response to treatment with IL-6 (100 ng/ml) alone or after pretreatment with PIC (P/IL-6) or AG490 (A/IL-6). Significance levels were established by comparing the different treatments to untreated (Ud) K562 cells. A representative Western blot probed with Stat3-specific polyclonal antibody that detects total Stat3 $alpha$ (t-Stat3 $alpha$ , 89 kDa) and Stat3 $beta$ (80 kDa) is shown. The graph shows the quantitative data obtained for the band intensities measured by SigmaGel Imaging software. Stat3 $alpha$ (white bars) and Stat3 $beta$ (black bars) levels are shown after IL-6 alone or after pretreatment with PIC (P/IL-6) or AG490 (A/IL-6).

Furthermore, the level of activated Stat3 $beta$ (phosphorylated) was greater than activated Stat3 $alpha$ at steady state. In time courseexperiments we observed a transient deactivation of both Stat3variants by IL-6 for up to 4 h. This was replaced by a rapid risein the level of activated Stat3 $beta$ reaching a maximal value at 24h, and remaining above base-line values for up to 48 h (data notshown). In contrast, deactivation of Stat3 $alpha$ was progressive throughoutthe study period. Consequently, the ratio of activated Stat3 $beta$ /Stat3 $alpha$ at 48 h was higher compared with untreated cells. This indicatesthat Stat3 $beta$ is the primary signaling protein mediating the effectof IL-6 in K562cells.

Stat3 Binds a Consensus Sequence in the $gamma$ Promoter-- A computer-aided search revealed a Stat3-like binding sequence (TTCTGGAA) in the A $gamma$ and G $gamma$ promoters, in the interval betweennucleotides +9 to +16 relative to the cap site, which is similarin structure to the Stat3 consensus sequence TT(N)_4-5AA(27, 28). DNA sequence alignment of the $beta$ -like globin genesshowed that the embryonic ( $epsilon$ ) globin gene lacked the terminalAA dinucleotide critical for Stat3 binding (Fig. 3A). In the twoadult globin genes ( $delta$ and $beta$ ) the octamer sequence terminates witha CA dinucleotide (Fig. 3A). We investigated potential DNA-proteininteractions in this region for each globin promoter using oligonucleotidesprobes spanning nucleotides +1 to +22. We observed two complexesof variable intensities with each radiolabeled probe and nuclearextract from K562 cells (Fig. 3B). Competition experiments withself and consensus Stat3 oligonucleotides suggest each promoter, $epsilon$ (lanes 2 and 3), $beta$ (lanes 5 and 6), and $gamma$ (lanes 7-9), may interactwith Stat3. However, the motif in the $gamma$ -globin promoter is themost closely related to the Stat3 consensus, and in competitionexperiments a consensus Stat3 oligonucleotide was most effectiveagainst the $gamma$ probe (lane 9).

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Fig. 3. Stat3-like binding sites are located in the 5'-untranslated regions of the $beta$ -like globin genes. A, the DNA sequence is shown from +1 to +22 relative to the respective cap sites for $epsilon$ -globin ( $epsilon$ 5U), G $gamma$ -globin (G $gamma$ 5U), A $gamma$ -globin (A $gamma$ STAT3), $delta$ -globin ( $delta$ 5U), and $beta$ -globin ( $beta$ 5U). The Stat3-like sites are underlined. The Stat3 site studied in detail in the A $gamma$ promoter is shown in the box. B, gel mobility shift assay was performed with ³²P-radiolabeled $epsilon$ 5U, $beta$ 5U, and A $gamma$ STAT3 probes and untreated K562 nuclear extract (4 µg) for all experiments. The cold competitors were added at 50-fold excess before adding radiolabeled probes. Complexes were resolved on a 4% non-denaturing polyacrylamide gel. $epsilon$ , $epsilon$ 5U; $beta$ , $beta$ 5U; A $gamma$ , A $gamma$ STAT3; S3, Stat3 cold competitor. See "Experimental Procedures" for Stat3 sequence.

DNA-protein interaction with the $gamma$ -globin probe (A $gamma$ STAT3) was competed by a Stat1 consensus oligonucleotide as well (Fig.4A, lanes 1-3) suggesting that Stat1 and Stat3 might bind as aheterodimeric complex to this region in the $gamma$ -globin promoter.Unlabeled A $gamma$ STAT3 oligonucleotide successfully competed for bindingwith consensus Stat3 and Stat1 probes (Fig. 4A, lanes 5-10). TheStat1 probe formed two major and two variable minor complexes(lane 8). A $gamma$ STAT3 specifically abolished the Band 2 DNA-proteincomplexes formed with the Stat3 and Stat1 probes. In addition,we observe a new faster mobility complex in competition experimentsbetween the Stat1 probe and A $gamma$ STAT3 cold competitor (Band 3, lane10). Subsequent experiments to confirm Stat3 binding were performedusing untreated K562 nuclear extract and anti-Stat3 or anti-Stat1antibodies (see "Experimental Procedures"). In both instancesthe addition of antibodies reproducibly abolished formation ofthe Band 2 complex (Fig. 4, lanes 1-3). This confirms that Stat1and Stat3 bind to the interval +1 to +22 containing a Stat3-likeelement in the $gamma$ -globin gene.

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Fig. 4. Stat3 binds in the A $gamma$ promoter 5'-untranslated region. A, EMSA showing competition experiments with the A $gamma$ STAT3 and control Stat3 and Stat1 consensus oligonucleotides is shown. Studies were performed with untreated K562 nuclear extract and 50-fold excess cold competitor. S1, Stat1. Other abbreviations are as in Fig. 3. B, EMSA was performed with Stat3 and Stat1 antibodies to demonstrate direct binding to A $gamma$ STAT3. The probe was preincubated with nuclear extract ( $-$ ) followed by the addition of 2 µg of polyclonal Stat3 antibodies (S3a) or Stat1 antibodies (S1a) overnight at 4 °C. EMSAs were also performed with nuclear extracts from K562 cells treated with IL-6 (100 ng/ml) or pretreated with AG490 (A/IL-6) or PIC (P/IL-6) followed by IL-6. See "Experimental Procedures" for more details.

To determine whether IL-6 treatment altered STAT protein interactions in the $gamma$ -globin promoter, we performed EMSA with nuclearextracts from K562 cells induced with IL-6 alone or followingpretreated with AG490 or PIC. Treatment with IL-6 alone produceda consistent increase in binding of nuclear proteins to the Band2 complex (lanes 1 and 4). This effect was reduced significantlyby PIC (lane 6) and AG490 to a lesser degree. Mutation analysisshowed a requirement for an intact Stat3-like motif in the A $gamma$ STAT3probe for nuclear protein binding. Formation of the Stat3-specificDNA-protein complex (Band 2) as well as a slower migrating complexwas abolished in a mutant A $gamma$ STAT3 oligonucleotide containing aCTG $right-arrow$ TGA substitution (nucleotides +11 to +13) (Fig. 5). An identicalmodification of the consensus Stat3 oligonucleotide produced anidentical result. Collectively, the JAK-STAT pathway inhibitorand DNA-protein binding experiments suggest a role for Stat3 $beta$ in $gamma$ -globin gene regulation.

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Fig. 5. Mutating the A $gamma$ STAT3-binding site abolished Stat3 binding. A, the DNA sequence for the three nucleotides mutated in the A $gamma$ STAT3 (mA $gamma$ ) probe compared with the wild-type and mutant Stat3 (mS3) oligonucleotides. B, EMSA showing the DNA-protein complexes established with untreated K562 nuclear extract and the wild-type (S3, A $gamma$ ) and mutant (mS3, mA $gamma$ ) probes.

The Inhibitory Effect of IL-6 Is Mediated through the Minimal $gamma$ Promoter-- The functional importance of Stat3 to $gamma$ -globin gene regulation was directly tested by transient transfection assays. In initialexperiments we found that IL-6 reduced the luciferase activityfrom an enhancerless construct, $gamma$ Luc, containing the minimum $gamma$ -globinpromoter ( $-$ 299 to +36) by 6-fold in transfected K562 cells after24 h of IL-6 treatment. This effect was abrogated when transfectedcells were pretreated with PIC prior to IL-6 treatment (data notshown). To accurately gauge the magnitude of the repressive effecton the $gamma$ promoter, subsequent experiments were performed witha construct containing the erythroid-specific enhancer HS2 ofthe $beta$ -globin locus control region upstream of the $-$ 299 promoter(HS2 $gamma$ Luc). As expected the luciferase activity from HS2 $gamma$ Luc was10-fold higher compared with that of the enhancerless construct.IL-6 reduced luciferase activity from the HS2 $gamma$ Luc reporter 8-fold(p < 0.05) (Fig. 6B). This result demonstrates that the powerfulHS2 enhancer failed to avert the repressive effect of IL-6 onthe $gamma$ promoter. Inhibition of Stat3 activation in transfectedK562 cells with PIC, however, restored luciferase activity tobase-line values. In control experiments, UO126, an extracellularreceptor kinase pathway inhibitor, showed no effect on IL-6-mediated $gamma$ promoter repression. These data provide evidence for the involvementof Stat3 in $gamma$ gene regulation.

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Fig. 6. Interleukin-6 mediates $gamma$ gene repression through the proximal promoter. A, schematic diagram of the luciferase reporter constructs studied. B, K562 cells were transfected with the $gamma$ Luc (white bar) or HS2 $gamma$ Luc (black bar) reporter constructs followed by IL-6 (100 ng/ml) treatment for 24 h (striped bars) in the absence or presence of PIC (10 µg/ml) or UO126 pretreatment for 30 min. Total protein was isolated and luciferase assay performed as outlined under "Experimental Procedures." The base plasmid PGL3-Basic was used as a positive control for transfection efficiency in all experiments. Luciferase activity for untreated (Ud) K562 cells was normalized to 1. C, K562 cells were transfected with the HS2 $gamma$ Luc plasmid alone (black bar) or followed by treatment with IL-6 alone or pretreatment with PIAS1 (P1) or PIAS3 (P3) antibody (10 µg/ml) for 2 h and then IL-6 for 24 h (striped bars). Total protein was isolated and luciferase assay performed as outlined under "Experimental Procedures." D, K562 cells were transfected with the HS2 $gamma$ Luc plasmid followed by NaB induction alone or pretreatment with P1 or P3 antibody for 2 h and then NaB (striped bars) for 24 h. Significance levels were established by comparing the different experimental conditions to untreated (Ud) K562 cells. Data represent the mean ± S.E.

Stat3 Inhibition by PIAS3 Antibody Reverses $gamma$ Gene Repression by IL-6-- We next sought to inhibit specifically the Stat3 transcription factor with protein inhibitors of activated STAT-3 (PIAS3)antibodies. PIAS are naturally occurring antibodies that directlyrepress phosphorylated STAT proteins (30, 31). TransfectedK562 cells were pretreated with PIAS1 or PIAS3 antibody (10 ng/ml)for 2 h followed by IL-6 treatment. The reduction in luciferaseactivity from the HS2 $gamma$ Luc construct in the presence of IL-6 wasunaffected by PIAS1 (Fig. 6C). In contrast, PIAS3 abolished thenegative effects of IL-6 on the HS2 $gamma$ Luc reporter and restoredluciferase activity to base-line levels. This result providesfurther evidence for the importance of Stat3 in silencing $gamma$ -globingene expression. Interestingly, in control experiments we foundthat PIAS3 reduced the luciferase activity in cells treated withNaB suggesting a requirement for Stat3 by NaB to augment $gamma$ promoteractivity (Fig. 6D). These diametric effects from general inhibitionof Stat3 are plausible given that the $alpha$ and $beta$ variants have opposingoutcomes on geneexpression.

Stat3 $beta$ Mediates $gamma$ Promoter Silencing through Its Cognate Downstream Binding Site-- Co-transfection experiments were performed with the HS2 $gamma$ Luc reporter and expression vectors for Stat3 $alpha$ (pS3 $alpha$ ) and Stat $beta$ (pS3 $beta$ )to provide a direct analysis of each transcription factor on $gamma$ promoter activity. Transfected K562 cells were cultured eitherin normal medium or in medium supplemented with IL-6 for maximalphosphorylation of Stat3 transcriptionfactors.

Stat3 $beta$ overexpression reduced luciferase activity by 20% in the absence of IL-6 and by a further 50% after activation withIL-6, compared with the levels observed in co-transfection experimentswith HS2 $gamma$ Luc and the corresponding empty expression vector (pSG5)(Fig. 7). Co-transfection of the reporter vector with pS3 $beta$ anda mutant Stat3 $alpha$ (pmS3 $alpha$ ) vector carrying a Y705F mutation blockedthe effects of pS3 $beta$ and restored luciferase activity to approximatelybase-line levels. Activation of the wild-type pS3 $alpha$ vector blockedthe repressive effect of endogenous Stat3 $beta$ on $gamma$ promoter activity,which was observed with the HS2 $gamma$ Luc reporter with the empty expressionvector (pcDNA3.1) (Fig. 7). The highest level of luciferase activity(5-fold above steady-state levels) was recorded in co-transfectionexperiments with the wild-type and mutant Stat3 $alpha$ expression vectors.

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Fig. 7. Stat3 proteins directly modulate $gamma$ promoter activity. Transient transfections were completed in K562 cells transfected with the HS2 $gamma$ Luc reporter alone or with the control base plasmids pSG5 and pDNA3.1. Experimental samples containing the expression vectors pStat3 $beta$ (pS3 $beta$ ) or pStat3 $alpha$ (pS3 $alpha$ ) either alone or with the mutant pStat3 $alpha$ (pmS3 $alpha$ ) vector were analyzed. Total DNA added was held constant at 30 µg. Transfected cells were grown for 24 h in the absence ( $-$ , white bars) or presence of IL-6 (+, black bars), and then total protein was harvested for luciferase assays as described under "Experimental Procedures." Luciferase activity was normalized for total protein, and pGL3 control activity was monitored with each transfection. The mean ± S.E. is shown.

The diametric effect of the two Stat3 transcription factors on $gamma$ promoter activity was confirmed by dose-response experiments.Fig. 8 shows that increasing Stat3 $beta$ expression progressively reducedluciferase activity for the wild-type HS2 $gamma$ Luc construct. The lowestlevel of activity (99% inhibition) was obtained by co-transfecting50 µg of the expression vector pS3 $beta$ with the reporter vector.In contrast, increasing the Stat3 $alpha$ expression vector to 50 µgstimulated luciferase activity to levels above base line in co-transfectionexperiments with HS2 $gamma$ Luc. Finally, co-transfection experimentswith pS3 $beta$ at a fixed concentration of 15 µg with increasing amountsof pS3 $alpha$ , from 10 to 50 µg (Fig. 8B), were completed. We observeda 10-fold concentration-dependent increase in $gamma$ promoter activityin the presence of IL-6 demonstrating the ability of Stat3 $alpha$ toovercome the repressive effect of Stat3 $beta$ .

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Fig. 8. Stat3 $beta$ acts as an inhibitor of $gamma$ promoter activity in a concentration-dependent manner. A, K562 cells were transfected with HS2 $gamma$ Luc alone or combined with pStat3 $beta$ (pS3 $beta$ ) or pStat3 $alpha$ (pS3 $alpha$ ) at concentrations from 10 to 50 µg (black and gray bars, respectively) in the presence of IL-6 for 24 h, and then luciferase activity was measured. B, co-transfection studies were completed with pS3 $beta$ at a concentration of 15 µg (black bar) and increasing pS3 $alpha$ from 10 to 50 µg (striped bars) for 24 h in the presence of IL-6 (+). A concentration-dependent derepression of $gamma$ promoter activity was observed with increasing amounts pS3 $alpha$ . Luciferase assays were performed as described under "Experimental Procedures." C, co-transfection studies were completed with the mutant HS2mt $gamma$ Luc reported carrying a CTG $right-arrow$ TGA mutation at +11 to +13 in the $gamma$ promoter, constructed by a PCR-based site-directed mutagenesis approach (see "Experimental Procedures"). Reporter plasmid at a concentration of 15 µg was co-transfected with 10-50 µg of pS3 $beta$ , and luciferase activity was measured at 24 h in the absence ( $-$ ) or presence or IL-6 (+).

Finally experiments were completed to determine whether the Stat3-binding site A $gamma$ STAT3 plays an important functional rolein Stat3 $beta$ -mediated $gamma$ gene silencing. By using site-directed mutagenesiswe constructed a reporter plasmid with the three nucleotides +11to +13 mutated (CTG $right-arrow$ TGA) to create HS2mtA $gamma$ Luc. The identicalbases were shown in Fig. 5 to be essential for Stat3 binding toA $gamma$ STAT3 by EMSA analysis. Most striking was the loss of IL-6-mediaterepression for HS2mtA $gamma$ Luc shown in Fig. 8C. Reporter activitywas decreased 20% for the mutant plasmid versus 80% inhibitionfor the wild-type HS2 $gamma$ Luc construct. With increasing amounts ofStat3 $beta$ , we no longer observed the concentration-dependent repressionof $gamma$ promoter activity, although some degree of repression atthe 20- and 30-µg concentrations did occur. Interestingly, thereporter activity for HS2mtA $gamma$ Luc returned to base-line levelsdespite the addition of up to 50 µg of Stat3 $beta$ . This is in contrastto the abolishment of $gamma$ promoter activity by 99% for the wild-typeHS2 $gamma$ Luc reporter (Fig. 8A, black bars). These studies providedirect evidence that the A $gamma$ STAT3 site plays an important rolein $gamma$ -globin silencing by Stat3 $beta$ .

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

We have demonstrated in this study that IL-6 reduces steady-state HbF synthesis in fetal erythroid progenitors thus corroboratingour observations made previously (6). Interestingly, IL-6 inhibitedthe proliferative capacity of fetal-stage progenitors contraryto what we observe routinely in cultures established with adulterythroid progenitors. This likely reflects phenotypic differencesamong erythroid progenitors from the two stages of development.Umbilical cord blood contains a larger pool of progenitors witha fetal pattern of globin gene expression, higher stem cell density,and engraftment capacity compared with progenitors from adultperipheral blood (32). Our results suggest that IL-6 elicitsfactors with distinct properties in fetal erythroid cells to regulatecell growth and globin generegulation.

Studies in transgenic mice indicate that $gamma$ -globin gene silencing in the adult stage is achieved primarily through competitionbetween the $beta$ - and $gamma$ -globin genes for activation by the locuscontrol region. Promoter elements with a more active role in globingene silencing containing cognate binding motifs for GATA-1 andYY-1 have been described in the $epsilon$ -globin gene at $-$ 208 and $-$ 269(33, 34). Interestingly, overexpression of GATA-1 in transgenicmice carrying the $beta$ -globin locus in a yeast artificial chromosomeresults in $epsilon$ -globin repression in both embryonic and adult erythroidcells (35). This suggests there is overlap in stage-specificand developmental stage-stable silencing mechanisms. A consensusYY1 site at $-$ 1086 (36), two direct repeat elements in the distalCCAAT box (37), and a GATA-1 site in the 5'-untranslated regionhave been identified in the $gamma$ -globin gene (29); however, theirrole in $gamma$ gene silencing has not been fully characterized. Inaddition to these regulatory elements we have identified a Stat3motif (TTCTGGAA) in the $gamma$ -globin 5'-untranslated region that isstructurally similar to the IL-6-rsponse element in the $alpha$ ₂-macroglobulingene (28). EMSA analysis in this study supports binding of aheterodimeric Stat1-Stat3 complex to A $gamma$ STAT3 during steady-state $gamma$ geneactivity.

The observation that Stat3-like binding sites are located in the analogous positions in the $epsilon$ -, $delta$ -, and $beta$ -globin genes lendfurther evidence for a physiologic role for STAT proteins in globingene regulation. In the $beta$ -globin 5'-untranslated region an importantregulatory element called the downstream core element is locatedat nucleotide +22, which binds transcription factor IID to augmenttranscription initiation (38). Naturally occurring mutationsidentified in this region produce a $beta$ -thalassemia phenotype inhumans (39). Whether STAT proteins alter transcription factorinteractions in this regulatory region remains to beelucidated.

A detailed analysis of the $gamma$ -globin promoter was completed to determine whether the repressive effect of IL-6 occurs at thestructural gene or cellular levels. The fact that Stat3 $beta$ was activatedat steady state and that IL-6 preferentially induced and phosphorylatedthis variant suggests Stat3 $beta$ serves as a more physiologicallyrelevant repressor of $gamma$ -globin. This conclusion was supportedby the Western blot data as well, which showed higher level activationfor Stat3 $beta$ in untreated K562 cells. Direct evidence that bothStat3 $alpha$ and Stat3 $beta$ are capable of altering $gamma$ promoter activitywas provided by co-transfection experiments. Stat3 $beta$ completelysilenced $gamma$ promoter activity in a concentration-dependent mannerfor the wild-type HS2 $gamma$ Luc plasmid. Mutating the A $gamma$ STAT3 site resultedin a loss of the concentration-dependent $gamma$ promoter repressionby Stat3 $beta$ at higher concentrations. The fact that inhibition wasseen at the lower Stat3 $beta$ concentrations suggests that other regulatoryelements are required to accomplish complete $gamma$ gene silencing.Finally we observed an opposite regulatory effect for Stat3 $alpha$ ,which enhanced $gamma$ promoter activity to overcome repression. Thisobservation is consistent with the transfection data for NaB-induced $gamma$ promoter activity, which was inhibited in the presence of PIAS3antibody. This supports the ability of NaB to induce Stat3 $alpha$ toactivate $gamma$ gene expression. Therefore, both Stat3 variants havephysiologically relevant roles in $gamma$ generegulation.

Possible mechanisms for $gamma$ gene silencing by STAT proteins are the formation of Stat3 $alpha$ /Stat3 $beta$ heterodimers or Stat3 $beta$ homodimers(11) that could serve as a dominant negative regulator whenbound to A $gamma$ STAT3 (Fig. 9). Caldenhoven et al. (11) demonstratedan increased affinity of Stat3 $beta$ over Stat3 $alpha$ for binding to theIL-6-response element to produce a net negative effect on geneexpression even in the presence of lower levels of the formervariant. Another potential mechanism for $gamma$ gene silencing is throughprotein-protein interactions. Although Stat3-like elements existat position +9 in all globin promoters, the G $gamma$ and A $gamma$ promotersare unique in that a second Stat3-like site is present betweenbases $-$ 6 and +3. Furthermore, a GATA-1 site is located at position+25 to +31, which has been shown to mediate $gamma$ gene repression(29). Preliminary EMSA analysis confirmed two DNA-protein complexesare established with the upstream Stat3-like sequence, similarto that observed for the consensus Stat3-binding site (data notshown). Stat3 $beta$ has been shown to interact with the AP-1 transcriptionfactor to activate $alpha$ ₂-macroglobulin gene activity in humans despitethe absence of a transactivation domain (16). In the $gamma$ promoter5'-untranslated region although no AP-1 sites are present, A $gamma$ STAT3is in close proximity to the GATA-1 site (Fig. 9) that represses $gamma$ promoter function (29). Activated Stat3 $beta$ may interact withGATA-1 to mediate its repressive effect. An alternative mechanismmight be the formation of a tetrameric Stat3 complex on the cognateA $gamma$ STAT3 and upstream Stat3-like sites to alter $gamma$ promoter activity.This type of interaction has been established for the $alpha$ ₂-macroglobulingene (28). Whether Stat3 proteins are capable of forming tetramericcomplexes and/or interacting with GATA-1 to achieve $gamma$ -globin genesilencing will be elucidated in future investigations.

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Fig. 9. Model for Stat3 interactions in the $gamma$ promoter target cis-regulatory element. Depicted is the $gamma$ promoter sequence contained in the HS2 $gamma$ Luc reporter plasmid. Five potential regulatory elements are clustered in the 5'-untranslated region including a Stat3-like sequence, AgStat3, the stage selector element (SSE)-like element, a GATA-1 site, and an A-T-rich sequence. The EMSA analysis presented in this study demonstrated Stat3 and Stat1 binding to the A $gamma$ STAT3 site, which overlaps the SSE-like element. After IL-6 induction Stat3 $beta$ increases and might form homodimers on its binding site to repress the $gamma$ promoter. Whether Stat3 $beta$ can interact with the Stat3-like sequence to form a tetrameric complex and/or the GATA-1 site via Stat3-GATA-1 heterodimers remains to be investigated. The $gamma$ -globin promoter is not drawn to scale.

	ACKNOWLEDGEMENT

We thank Heather Norris for clericalassistance.

	FOOTNOTES

^* This work was supported by National Institutes of Health Grant HL 38639 (to B. S. P.).The costs of publication of this articlewere defrayed in part by the payment of page charges. The articlemust therefore be hereby marked "advertisement" in accordancewith 18 U.S.C. Section 1734 solely to indicate thisfact.

To whom correspondence should be addressed: Dept. of Cell Biology and Neuroscience, University of South Alabama, 307 UniversityBlvd., MSB 2406, Mobile, AL 36688. Tel.: 334-460-6109; Fax: 334-460-6771;E-mail: bpace@usouthal.edu.

Published, JBC Papers in Press, February 20, 2002, DOI 10.1074/jbc.M106556200

ABBREVIATIONS

The abbreviations used are: STAT, signal transducers and activators of transcription; JAK, Janus kinase; IL-6, interleukin-6; PIC, piceatannol; NaB, sodium butyrate; BFU-E, burst-forming unit erythroid; HbF, fetal hemoglobin; RPA, RNase protection assay; GAPD, glyceraldehyde-3-phosphate dehydrogenase; HS2, hypersensitive site 2; EMSA, electrophoretic mobility shift assay; PIAS, protein inhibitors of activated STAT.

	REFERENCES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

1.	Taniguchi, T. (1995) Science 268, 251-255[Abstract/Free Full Text]
2.	Ihle, J. N., and Kerr, I. M. (1995) Trends Genet. 11, 69-74[CrossRef][Medline] [Order article via Infotrieve]
3.	Ihle, J., Witthuhn, B. A., Quelle, F. W., Yamamoto, K., and Silvennoinen, O. (1996) Annu. Rev. Immunol. 13, 369-398
4.	Auernhammer, C. J., Chesnokova, V., Bousquet, C., and Melmed, S. (1998) Mol. Endocrinol. 12, 954-961[Abstract/Free Full Text]
5.	Helman, D., Sandowski, Y., Cohen, Y., Matsumoto, A., Yoshimyra, A., Merchav, S., and Gertler, A. (1998) FEBS Lett. 441, 287-291[CrossRef][Medline] [Order article via Infotrieve]
6.	Ferry, A., Baliga, S., Monterio, C., and Pace, B. S. (1997) J. Biol. Chem. 272, 20030-20037[Abstract/Free Full Text]
7.	Evans, T., Felsenfeld, G., and Reitman, M. (1990) Annu. Rev. Cell Biol. 6, 95-124[CrossRef][Medline] [Order article via Infotrieve]
8.	Orkin, S. H. (1984) J. Biol. Chem. 270, 4955-4958
9.	Darnell, J. E., Jr. (1997) Science 277, 1630-1635[Abstract/Free Full Text]
10.	Hoey, T., and Schindler, U. (1998) Curr. Opin. Genet. Dev. 8, 582-587[CrossRef][Medline] [Order article via Infotrieve]
11.	Caldenhoven, E., van Dijk, T. B., Solari, R., Armstrong, J., Raaijmakers, J. A. M., Lammers, J. J., Koenderman, L., and de Groot, R. P. (1996) J. Biol. Chem. 271, 13221-13227[Abstract/Free Full Text]
12.	Wen, Z., and Darnell, J. E., Jr. (1997) Nucleic Acids Res. 25, 2062-2067[Abstract/Free Full Text]
13.	Wen, Z., Zhong, Z., and Darnell, J. E., Jr. (1995) Cell 82, 241-250[CrossRef][Medline] [Order article via Infotrieve]
14.	Shuai, K. (2000) Oncogene 19, 2638-2644[CrossRef][Medline] [Order article via Infotrieve]
15.	Schaefer, T. S., Sanders, L. K., Park, O. E., and Nathans, D. (1997) Mol. Cell. Biol. 17, 5307-5316[Abstract]
16.	Schaefer, T. S., Sanders, L. K., and Nathans, D. (1995) Proc. Natl. Acad. Sci. U. S. A. 92, 9097-9101[Abstract/Free Full Text]
17.	Yang, Y., Pace, B. S., Kitchens, D., Ballas, S. K., Shah, A., and Baliga, B. S. (1997) Am. J. Hematol. 56, 252-258[CrossRef][Medline] [Order article via Infotrieve]
18.	Baliga, B. S., Pace, B. S., Chen, H., Shah, A. K., and Yang, Y. (2001) Am. J. Hematol. 65, 227-233
19.	Pace, B. S., Chen, Y. R., Thompson, A., and Goodman, S. R. (2001) Exp. Hematol. 28, 283-293
20.	Andrews, N. C., and Faller, D. V. (1991) Nucleic Acids Res. 19, 2499[Free Full Text]
21.	Levitzki, A. (1990) Biochem. Pharmacol. 40, 913-918[CrossRef][Medline] [Order article via Infotrieve]
22.	Geahlen, R. L., and McLaughlin, J. L. (1989) Biochem. Biophys. Res. Commun. 165, 214-245[CrossRef]
23.	Seidel, H. M., Milocco, L. H., Lamb, P., Darnell, J. E., Jr., Stein, R. B., and Rosen, J. (1995) Proc. Natl. Acad. Sci. U. S. A. 92, 3041-3045[Abstract/Free F

Stat3 Inhibits -Globin Gene Expression in Erythroid Cells*

Stat3 $beta$ Inhibits $gamma$ -Globin Gene Expression in Erythroid Cells^*