ETO, but Not Leukemogenic Fusion Protein AML1/ETO, Augments RBP-J{kappa}/SHARP-Mediated Repression of Notch Target Genes

Notch is a transmembrane receptor that determines cell fatesand pattern formation in all animal species. After specificligand binding, the intracellular part of Notch is cleaved offand translocates to the nucleus, where it targets the DNA bindingprotein RBP-J ${kappa}$ . In the absence of Notch, RBP-J ${kappa}$ represses Notchtarget genes by recruiting a corepressor complex. We and othershave previously identified SHARP as one component of this complex.Here, we show that the corepressor ETO as well as the leukemogenicfusion protein AML1/ETO directly interacts with SHARP, thatETO is part of the endogenous RBP-J ${kappa}$ -containing corepressor complex,and that ETO is found at Notch target gene promoters. In functionalassays, corepressor ETO, but not AML1/ETO, augments SHARP-mediatedrepression in an histone deacetylase-dependent manner. Furthermore,either the knockdown of ETO or the overexpression of AML1/ETOactivates Notch target genes. Therefore, we propose that AML1/ETOcan disturb the normal, repressive function of ETO at Notchtarget genes. This activating (or derepressing) effect of AML1/ETOmay contribute to its oncogenic potential in myeloid leukemia.

INTRODUCTION

Top

INTRODUCTION

A small number of signaling pathways are known to regulate geneexpression and, hence, cell fates in many organ systems. Notchacts as the receptor in one of these pathways and is involvedin regulating many cellular processes, such as stem cell maintenanceor differentiation during the development and renewal of adulttissues (reviewed in references 5 and 17). In higher eukaryotes,well-studied examples of the influence of Notch on cell fateare neurogenesis and myogenesis in Drosophila (reviewed in reference4) and hematopoiesis in mice (reviewed in references 27 and38).

At the molecular level, the triggering of the Notch receptorby ligand binding leads to proteolytic processing within thetransmembrane domain, which results in the release of the Notchintracellular domain Notch-IC. Notch-IC can translocate to thenucleus, where it targets the DNA binding protein RBP-J ${kappa}$ , alsoknown as CSL [CBF1, Su(H), Lag-1)], in order to activate Notchtarget genes. In mice and Drosophila melanogaster, the phenotypesthat are produced upon depletion of RBP-J ${kappa}$ are similar, but notidentical, to those produced by the loss of Notch function.Subsequently, it became clear to us that many differences couldbe explained by the derepression of Notch target genes. Hence,we postulated that repression and activation via RBP-J ${kappa}$ involvethe recruitment of distinct corepressors and coactivator complexes(reviewed in references 5 and 23). Notch-IC binding to RBP-J ${kappa}$ is crucial for switching from the repressed state to the activatedstate. When Notch-IC enters the nucleus, its binding to RBP-J ${kappa}$ may trigger an allosteric change that facilitates the displacementof the transcriptional corepressor complex. Subsequently, Mastermindbinds to Notch-IC/RBP-J ${kappa}$ and the resulting ternary protein complexrecruits coactivators, such as histone acetyltransferase p300or PCAF (22, 33, 40, 44), chromatin remodeling factors, andthe mediator complex, to activate transcription (12). When Notch-ICis absent from the nucleus, RBP-J ${kappa}$ recruits a histone deacetylase(HDAC)-containing corepressor complex (15, 18, 32, 34).

We and others have previously described the protein SHARP (SMRT-and HDAC1-associated repressor protein) as part of the RBP-J ${kappa}$ corepressor complex (21, 32). SHARP is a ubiquitously expressed,large protein of approximately 450 kDa, containing four RNArecognition motifs at its N terminus and a highly conservedSPOC domain at its C terminus (3, 30, 37). Its highly conservedrepression domain has been described to interact with SMRT andN-CoR (37) and with CtIP/CtBP (34). Mice deficient for the murineSHARP homologue MINT die during late embryogenesis (21). Studiesusing fetal liver transfer and a conditional knockout approachhave shown a SHARP deficiency to cause hematopoietic defectsin marginal zone B-cell development and T-cell development (21,39, 45).

ETO (also called myeloid translocational gene 8 protein [MTG8])is best known as a fusion partner of AML1 in leukemias carryingthe t(8;21) translocation (10, 29); in fact, the name of theprotein is an acronym for the translocation (eight-twenty-one).ETO belongs to a family of conserved nuclear proteins whosemembers can be found from Drosophila to humans. It containsfour evolutionarily conserved functional domains called nervyhomology regions (NHRs). NHR2 is important for homodimerizationand protein-protein interaction with other corepressors. AlthoughETO is not able to bind to DNA, it is reported to act as a negativetranscriptional regulator. ETO can homodimerize and heterodimerizewith other members of the ETO family as well as interact directlywith the corepressors N-CoR, SMRT, and Sin3A (reviewed in reference16) (13, 26, 41). The function of ETO as a corepressor dependsalso on recruitment of HDACs, especially HDAC1, -2, and -3 (2).

The t(8;21)(q22/q22) translocation, which fuses the ETO geneon human chromosome 8 with the AML1 gene on chromosome 21, isseen in approximately 12 to 15% of acute myeloid leukemia (AML)cases, and in about 40% of AML cases, it is seen with a French-American-British-classifiedM2 phenotype (9). AML1 (also known as Runx-1) is a transcriptionfactor that forms a heterodimer with a non-DNA-binding protein,CBFβ (31, 41). The t(8;21) translocation fuses DNA encodingthe N-terminal 177 amino acids of AML1, which includes the RUNTDNA-binding domain (which also interacts with CBFβ), inframe with the codons for amino acids 30 to 604 of ETO. TheAML1/ETO fusion deletes the terminal activation domain of AML1and acts as a dominant-negative form of AML1, which repressesAML1 target genes. In contrast, AML1/ETO could also be foundas an activator of transcription involving Bcl-2 (20) and enhancedthe expression of p21^WAF1 (35). However, the mechanism throughwhich AML1/ETO can activate transcription remains unclear.

The focus of this study is to further characterize the RBP-J ${kappa}$ /SHARPcorepressor complex. In a yeast two-hybrid screen with the RBP-J ${kappa}$ -interactingcorepressor SHARP, ETO was identified as an interaction partner.SHARP-ETO interaction was confirmed in glutathione S-transferase(GST) pull-down and coimmunoprecipitation experiments. Furthermore,in chromatin immunoprecipitation (ChIP) experiments, the colocalizationof RBP-J ${kappa}$ /SHARP and ETO could be found at Notch target genes.Interestingly, the leukemogenic fusion protein AML1/ETO alsointeracts with SHARP and is present in the endogenous RBP-J ${kappa}$ corepressor complex of Kasumi cells. However, in functionalassays, ETO but not AML1/ETO augments SHARP-mediated repression.Moreover, AML1/ETO is able to disturb transcriptional repressionat Notch target genes. Therefore, we propose that AML1/ETO deregulatesnot only AML1 target genes but also Notch target genes.

MATERIALS AND METHODS

Top

MATERIALS AND METHODS

Oligonucleotides. For a list of all oligonucleotides used for the constructionof plasmids and for real-time PCR, see the materials and methodssection of the supplemental material.

Plasmids. The ETO expression plasmid was made by inserting the SalI (bluntedwith Klenow fragment)-digested/NotI-digested ETO fragment frompBind-ETO (provided by J. Lausen) into the EcoRV-digested/NotI-digestedpDNA3 vector. The AML1/ETO expression plasmid was produced frompGEX6P1-AML1/ETO (provided by J. Lausen) in a manner similarto that described above. For bacterial expression of GST fusionproteins, the KpnI (blunted with Klenow fragment)-digested/NotI-digestedETO fragment from pcDNA3-ETO was inserted into the SmaI-digested/NotI-digestedpGEX6P1 vector (Amersham). The GST fusions of SHARP as wellas the expression plasmids pcDNA3-Flag-SHARP-RD and pcDNA3-Flag2-SHARPhave previously been described (32, 34). For mapping of theSHARP ETO interaction, the expression plasmids pcDNA3-Flag3-ETO-N(amino acids 1 to 305), pcDNA3-Flag3-ETO-C (amino acids 297to 604), and pcDNA3-Flag3-ETO (amino acids 400 to 604) wereconstructed as follows. The N-terminal fragment of ETO (ETO-N)was amplified by PCR using ETO-N_001 and ETO-N_002 as primers,digested with EcoRI and XhoI, and inserted into the correspondingsites of pcDNA3-Flag3. The C terminus of ETO (ETO-C) was amplifiedusing the primers ETO-C_001 and ETO-C_002, digested with EcoRVand XhoI, and inserted into the corresponding sites of pcDNA3-Flag3.The ETO deletion mutant (amino acids 400 to 604) was amplifiedusing the primers ETO-del_001 and ETO-del_002 by PCR, digestedwith EcoRV and XhoI, and inserted into pcDNA3-Flag3. The pcDNA3-ETO-enhancedgreen fluorescent protein (eGFP) and pcDNA3-AML1/ETO-eGFP constructswere made as follows. ETO-C was amplified by PCR using the upstreamprimer ETO_001 and the downstream primer ETO_002, digested withEcoRI and XhoI, and inserted into the corresponding sites ofpcDNA3-eGFP, resulting in pcDNA3-ETO-C-eGFP. For inserting theN-terminal part of ETO or AML1/ETO, the vectors pcDNA3-ETO andpcDNA3-AML1/ETO were digested with EcoRI and inserted into thecorresponding site of pcDNA3-ETO-C-eGFP. The pcDNA3-Flag3-AML1/ETO(tr)-eGFPexpression plasmid was produced as follows. The C-terminal partof AML1/ETO was deleted using the 5' phosphorylated oligonucleotidesTR_001 and TR_002. The oligonucleotides were annealed, and theresulting double-stranded DNA flanked by the restriction sitesfor BamHI and XhoI was inserted into the corresponding sitesof pcDNA3-Flag3-AML1/ETO, resulting in pcDNA3-Flag3-AML1/ETO(tr).For eGFP fusion, pcDNA3-AML1/ETO-eGFP was digested with XhoIand XbaI and the eGFP sequence was inserted into the correspondingsites of pcDNA3-Flag3-AML1/ETO(tr). The RBP2N specific expressionvector pcDNA3-RBP2N-d2EosFP (42) was digested with XhoI andXbaI, and the PCR-amplified eqFP611 cDNA (primers RBP_001 andRBP_002) was inserted, resulting in RBP2N-eqFP611. The reporterplasmids for the luciferase assays pFR-Luc, pGA981/6, and HES1-Lucas well as the expression plasmids pCMV-RBP-VP16, pCMV-Gal4-VP16-SHARP-RD,pCMV-mNotch-1-IC, and pcDNA3-Flag1-SHARP (amino acids 2770 to3127) were described previously (32). The Hey1(–97/+85)-Lucreporter was a gift from M. Gessler. The ETO(xl) and XETOR expressionplasmids were gifts from Ying Cao, University of Ulm.

Yeast two-hybrid screening. Yeast two-hybrid screening was performed as described previously(32).

Cell culture and preparation of cell extracts. The HEK293 (ATCC CRL 1573) and HeLa (ATCC CCL 2) cell lineswere grown in Dulbecco's modified Eagle's medium (Gibco) supplementedwith 10% fetal calf serum (FCS). The Kasumi cell line was grownin RPMI 1640 medium (Gibco) supplemented with 20% FCS, 5% HEPES,and 5% L-glutamine. The murine erythroleukemia (MEL) and humanerythroleukemia (HEL) cell lines were grown in RPMI 1640 medium(Gibco) with 10% FCS, penicillin, and streptomycin. A pre-T-cellline called Beko was derived from mice deficient in T-cell receptorbeta (kind gift from J. Kisielow). Beko cells were grown inIscove's modified Dulbecco medium (Gibco) with 2% FCS, nonessentialamino acids, 0.3 mg/liter Primatone, and 5 mg/liter insulin.All cell lines were maintained at 37°C under 5% CO₂. Whole-celllysates for Western blotting and immunoprecipitation experimentswere prepared as follows. Cells were washed in phosphate-bufferedsaline (PBS) and suspended in ice-cold CHAPS lysis buffer (10mM 3{3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonate},50 mM Tris-HCl, pH 7.8, 150 mM NaCl, 5 mM NaF, 0.5 mM phenylmethylsulfonylfluoride and protease inhibitors; Complete mix; Roche) and incubatedon ice for 1 h. The lysates were cleared by centrifugation at80,000 x g for 30 min. Protein concentrations were determinedby using the Bradford assay method (Bio-Rad). The extracts wereused for Western blotting and immunoprecipitation experiments.

DNA transfection. HEK293 cells were transfected using the calcium phosphate coprecipitationmethod (Promega), HeLa cells were transfected using the FuGENEtransfection reagent (Roche), and Kasumi cells were transfectedwith Lipofectamine 2000 (Invitrogen). All transfections wereperformed according to the manufacturer's instructions.

In vitro protein translation. Proteins were translated in vitro in the presence of [³⁵S]methionineby using the reticulocyte lysate-coupled transcription/translationsystem (Promega). Translation and labeling quality were monitoredby sodium dodecyl sulfate-polyacrylamide gel electrophoresis(SDS-PAGE).

GST pull-down assay. The GST fusion proteins were expressed in Escherichia coli strainBL21 (Stratagene) and stored as whole bacterial lysates at –80°C.Approximately 1 µg of GST protein and GST fusion proteinwere immobilized with glutathione-Sepharose beads (Amersham)and incubated together with the in vitro-translated proteinsunder rotation at 4°C for 1 h. Beads were washed four timeswith 600 µl buffer A (40 mM HEPES [pH 7.5], 5 mM MgCl₂,0.2 mM EDTA, 0.5% NP-40, and 100 mM KCl) and four times with600 µl buffer B (equivalent to buffer A, but containing300 mM KCl). After the washing steps, the beads were resuspendedin SDS-PAGE loading buffer and the proteins were separated bySDS-PAGE. The gels were dried and exposed to X-ray films.

Immunoprecipitation. Immunoprecipitation experiments were carried out using whole-cellextracts from HEK293 cells 24 h after cotransfection with Flag-SHARP-RD(3477 to 3664) and expression plasmids for ETO and AML1/ETO.Cells were lysed with 700 µl CHAPS lysis buffer. The extractswere incubated with 40 µl agarose-conjugated anti-Flagantibody (M2; Sigma) at 4°C overnight. The beads were washedfive times with CHAPS lysis buffer and resuspended in SDS-polyacrylamidegel loading buffer. For the investigation of endogenous proteininteractions, immunoprecipitation experiments were carried outusing CHAPS cell extracts from Kasumi cells or HEL cells. Theextracts were incubated with 4 µg of anti-ETO antibody(Santa Cruz) or 20 µl of an anti-SHARP antibody ( ${alpha}$ SHARP2 [32]) at 4°C overnight, followed by a 2-h incubation with40 µl Sepharose-conjugated protein G beads (Amersham).The beads were washed five times with CHAPS lysis buffer andresuspended in SDS-PAGE loading buffer.

Western blotting. The proteins resolved in SDS-polyacrylamide gels (10%) weretransferred electrophoretically at room temperature to polyvinylidenedifluoride membranes (Millipore) for 1 h at 50 mA by using aTris-glycine buffer system. The membranes were preblocked for1 h in a solution of 2% or 3% milk powder in 0.1% Tween 20 inPBS (PBS-T) before the antibodies were added. The followingantibodies were used: anti-ETO (goat polyclonal immunoglobulinG [IgG] raised against the C terminus of ETO; catalog no. sc-9737;Santa Cruz), secondary antibody peroxidase-conjugated rabbitanti-goat IgG (Jackson ImmunoResearch), anti-Flag (catalog no.M5; Sigma), secondary antibody peroxidase-conjugated sheep anti-mouseIgG (catalog no. NXA931; Amersham), anti-RBP-J ${kappa}$ (rat monoclonalIgG2a [catalog no. T6709; Institute of Immunology Co., Ltd.]and secondary antibody peroxidase-conjugated goat anti-rat IgG[Dianova]), anti-VP16 (mouse monoclonal IgG directed againstamino acids 456 to 490 of VP16 [catalog no. sc-7545; Santa Cruz]and secondary antibody peroxidase-conjugated sheep anti-mouseIgG [NXA931; Amersham]).

Luciferase assay. HeLa cells (5 x 10⁴) were transfected in 24-well plates (with1 µg of reporter plasmid DNA), together with various amountsof expression plasmid. Luciferase activity was determined fromat least three independent transfections with 20 µl ofcleared lysate in an LB 9501 luminometer (Berthold) by usingthe luciferase assay system from Promega.

Purification of RBP-J ${kappa}$ DNA-binding complexes. Purification was performed as described previously (34). Whole-cellextracts from 10⁹ Kasumi cells were used. The DNA-binding complexeswere analyzed by electromobility shift assay (EMSA) and Westernblotting.

EMSA. The EMSA experiments were performed as described previously(34).

ChIP. MEL and Kasumi cells were fixed for 1 h with 10 mM dimethyladipimate.For cross-linking, the cells were incubated in 1% formaldehydefor 10 min at room temperature. The cross-linking reaction wasstopped with 125 mM glycine. Nuclear extracts were preparedby using a cell lysis buffer (50 mM Tris-HCl [pH 8.0], 2 mMEDTA, 0.1% NP-40, 10% glycerol, 2 mm dithiothreitol). The nucleiwere resuspended in 600 µl resuspension buffer (50 mMTris-HCl [pH 8.0], 1% SDS, 5 mM EDTA, 2 mM dithiothreitol) andsonicated. Chromatin was 10-fold diluted with dilution buffer(50 mM Tris-HCl [pH 8.0], 200 mM NaCl, 5 mM EDTA, 0.5% NP-40)and precleared. The precleared chromatin extract was incubatedovernight with, in each case, 50 µg antibodies againstETO (rabbit polyclonal antibody), SHARP (rabbit polyclonal antibody),and RBP-J ${kappa}$ (Chemicon). The immunoprecipitates were immobilizedon protein A-Sepharose beads for 2 h. After washing the beadswith 500 mM NaCl and 500 mM LiCl containing buffers, we elutedchromatin from the beads with elution buffer (Tris-EDTA, 2%SDS) at room temperature. The cross-linking of chromatin wasreversed for 6 h at 65°C in the presence of 300 mM NaCland RNase A. Chromatin was precipitated with ethanol, dissolvedin Tris-EDTA-PK buffer (10 mM Tris-HCl [pH 7.5], 5 mM EDTA,0.25% SDS) and treated with proteinase K for 2 h at 45°C.After purification by phenol-chloroform extraction, the chromatinwas precipitated at –20°C in the presence of 300 mMNaCl, tRNA, glycogen, and ethanol overnight. The chromatin wasanalyzed by quantitative real-time PCR.

Overexpression in HEK293 cells and knockdown in Kasumi and pre-T cells. HEK293 cells (3 x 10⁶ in 10-cm dishes) were transfected withan empty pcDNA3 vector or expression plasmids pcDNA3-AML1/ETO,pcDNA3-AML1/ETO(tr), pcDNA3-mNotch-1-IC, and pCMV-RBP-VP16.The cells were harvested 24 h after transfection. After mRNAisolation and cDNA synthesis, the expression of Notch targetgenes was determined by real-time PCR. Kasumi cells were transfectedwith the pSIR-short interfering RNA (siRNA)-internal ribosomeentry site-GFP vector, which expresses the specific AML1/ETOjunction hairpin (CGA GAA CCU CGA AAU CGU ACT). GFP-positiveand GFP-negative cells were sorted by fluorescence-activatedcell sorting 3 days after transfection and subsequently analyzedvia reverse transcription-PCR. The pre-T-cell line Beko wasretrovirally infected with the pSIR-siRNA-histidinol vector,which expresses either hairpin ETO1.1 (GCA TGA GCA CCT TCT GCTCAA) or hairpin ETO1.2 (GAT CGC CTG TGG AAG TGA AGA). The retroviralpackaging cell line Phoenix was transfected with calcium phosphate.Two days later, retroviral supernatants were taken and Bekocells were spin infected four times over 2 days. Cells wereselected on 500 mM histidinol, and real-time PCR was performed1 week after selection.

RESULTS

Top

RESULTS

Corepressor SHARP physically interacts and colocalizes with ETO and AML1/ETO. In order to identify proteins that interact with the RBP-J ${kappa}$ -associatedcorepressor SHARP, we performed a yeast two-hybrid screen byusing the repression domain of SHARP (SHARP-RD) as bait. A humanembryonic brain library was screened, and the corepressor ETOwas identified as an interactor. The association between SHARP-RDand ETO was verified in several independent assays (Fig. 1 and2). First, in GST pull-down experiments, full-length ETO, radiolabeledin a cell-free system, interacted only with the bacteriallyexpressed GST fusion protein GST-SHARP-RD (amino acids 3477to 3664) (Fig. 1A, lane 4), not with a C-terminally truncatedmutant of GST-SHARP-RD (amino acids 3477 to 3628) or GST alone(Fig. 1A, lanes 2 and 3). The fusion protein AML1/ETO, containingalmost the whole ETO protein fused to the DNA-binding domainof AML1, also bound only to GST-SHARP-RD (amino acids 3477 to3664) (Fig. 1B, lane 4), not to the truncated GST-SHARP-RD (aminoacids 3477 to 3628) or GST alone (Fig. 1B, lanes 2 and 3).

View larger version (77K):
[in this window]
[in a new window]

FIG. 1. ETO and AML1/ETO interact with SHARP in vitro (A and B) and in vivo (C and D). (A and B, lanes 4) Cell-free, synthesized, ³⁵S-labeled ETO and AML1/ETO bind to GST-tagged SHARP-RD (amino acids 3477 to 3664) immobilized on glutathione-Sepharose beads. (A and B, lanes 3) They do not interact with a truncated version of immobilized GST-SHARP-RD (amino acids 3477 to 3628). (C) HEK293 cells were cotransfected with expression plasmids for ETO or AML1/ETO, together with Flag-tagged SHARP-RD. The expression of Flag-SHARP-RD, ETO, and AML1/ETO was detected by Western blotting (WB) using antibodies against the Flag tag (upper blot) and ETO (middle blot). ETO and AML1/ETO were coimmunoprecipitated only with SHARP-RD from lysates of cells cotransfected together with Flag-SHARP-RD (lower blot, lanes 4 and 5). (D) Endogenous RBP-J ${kappa}$ and ETO could be coimmunoprecipitated from HEL cellular extracts by an anti-SHARP antibody (lanes 3 and 4). Coimmunoprecipitated ETO and AML1/ETO were detected on Western blots using the ETO antibody ( ${alpha}$ ETO). Coimmunoprecipitated RBP-J ${kappa}$ was detected using the RBP-J ${kappa}$ antibody ( ${alpha}$ RBP-J ${kappa}$ ).

View larger version (42K):
[in this window]
[in a new window]

FIG. 2. The first two functional domains of ETO (NHR1 and NHR2) are responsible for interaction with SHARP-RD. (A) Schematic representation of ETO and the truncated versions of ETO used in this study. (B) GST pull-down with the cell-free, synthesized, Flag-tagged, N-terminal (amino acids 1 to 305) and C-terminal (amino acids 297 to 604) halves of ETO. Both interact only with GST-SHARP-RD (amino acids 3477 to 3664) (lanes 5 and 8), not with the truncated GST-SHARP-RD (amino acids 3477 to 3628) (lanes 4 and 7) or GST alone (lanes 3 and 6). The GST fusions were immobilized on glutathione-Sepharose beads. (C) Cell-free synthesized ETO (amino acids 400 to 604) does not bind to immobilized GST-SHARP-RD any more (lanes 4 and 5). Cell-free synthesized full-length ETO was used as positive control (lane 6).

Secondly, coimmunoprecipitation experiments were performed inorder to confirm the interaction of ETO (or AML1/ETO) and SHARP-RDin vivo. For this purpose, HEK293 cells were transiently transfectedwith expression plasmids for ETO or AML1/ETO alone or togetherwith Flag-tagged SHARP-RD. Flag-SHARP-RD was immunoprecipitatedwith an anti-Flag antibody; ETO and AML1/ETO were detected inWestern blot analyses by using an anti-ETO antibody (Fig. 1C).Immunoprecipitated ETO and AML1/ETO could be detected only ifthey were expressed together with Flag-SHARP-RD (Fig. 1C, bottompanel). In addition, after the incubation of cell lysates fromETO-expressing HEL cells (Fig. 1D, lane 2) with an antibodydirected against endogenous SHARP protein (32), both RBP-J ${kappa}$ (Fig.1D, lane 3) and ETO (Fig. 1D, lane 4) were coimmunoprecipitated.

ETO contains four highly conserved functional domains callednervy homology regions (NHR1 to NHR4). Previous investigationsshowed that these domains mediate interaction with other repressorproteins like N-CoR, SMRT, or Sin3A (2, 25, 26, 41). In orderto identify which domains of ETO are responsible for SHARP interaction,several Flag-tagged, truncated versions of ETO were synthesized(Fig. 2A). Both the N-terminal part of ETO containing NHR1,Flag3-ETO-N (amino acids 1 to 305), and the C-terminal part,Flag3-ETO-C (amino acids 297 to 604), containing NHR2 to NHR4,associated with GST-SHARP-RD (amino acids 3477 to 3664) in GSTpull-down experiments (Fig. 2B, lanes 5 and 8). Neither constructshowed any interaction with GST alone (Fig. 2B, lanes 3 and6) or with the truncated GST-SHARP-RD (amino acids 3477 to 3628)(Fig. 2B, lanes 4 and 7). In vitro-translated, Flag-tagged ETO(400 to 604) containing NHR3 and NHR4 was not able to bind toGST-SHARP-RD (amino acids 3477 to 3664) (Fig. 2C, lane 5) ina comparison with full-length ETO as a positive control (Fig.2C, lane 6). These results demonstrate that SHARP interactswith ETO and AML1/ETO in vitro and in vivo. Furthermore, thefirst two functional domains of ETO contribute to the interactionwith the full-length SHARP repression domain in a manner independentof each other.

Since, at the moment, it is not possible to detect SHARP byWestern blotting (21, 32), we decided to use an immunofluorescenceapproach. To examine the subcellular localization of SHARP,ETO, and AML1/ETO, HEK293 cells were cotransfected with eGFPfusions of ETO, AML1/ETO, and a recently identified C-terminallytruncated version of AML1/ETO (46), together with full-lengthSHARP (see Fig. S1A in the supplemental material). SHARP wasimmunostained using an anti-serum directed against SHARP. Allthree eGFP fusion proteins and SHARP locate to the nucleus (seeFig. S1A in the supplemental material). SHARP interacts withRBP-J ${kappa}$ through a conserved interaction domain (32). To investigatethe subcellular localization of SHARP, RBP-J ${kappa}$ , and AML1/ETO triple-colorfluorescence images were taken of the nuclei of HEK293 cellscotransfected with AML1/ETO-eGFP and a fusion of RBP2N withan optimized variant of the red fluorescent protein eqFP611(42, 43). AML1/ETO-eGFP, RBP2N-eqFP611, and endogenous SHARPlocalized in the nuclei of HEK293 cells (see Fig. S1B in thesupplemental material).

ETO and SHARP colocalize with RBP-J ${kappa}$ at promoter regions of Notch target genes. To investigate whether the ETO-SHARP interaction also takesplace at Notch target genes in vivo, ChIP experiments were performed.We used ETO-expressing MEL cells and investigated whether ETO,SHARP, and RBP-J ${kappa}$ can be found specifically at several Notchtarget gene promoters. After the immunoprecipitation of eitherRBP-J ${kappa}$ , SHARP, or ETO, promoter regions of the HES1 gene andof the newly described Notch target Nrarp (24) could be specificallyamplified, whereas several control regions (control 1, HES1gene 3' untranscribed region [UTR]; control 2, Hey1 gene 3'UTR) remained at background levels (Fig. 3).

View larger version (21K):
[in this window]
[in a new window]

FIG. 3. ETO, SHARP, and RBP-J ${kappa}$ can be found associated at the promoter regions of the Notch target HES1 and Nrarp genes in MEL cells. ChIP experiments were performed as described in Materials and Methods. Mean values and standard deviations (error bars) of four independent experiments are shown. Control 1, HES1 gene 3' UTR; control 2, Hey1 gene 3' UTR.

AML1/ETO is part of the endogenous RBP-J ${kappa}$ -complex. Previously, we isolated endogenous RBP-J ${kappa}$ -containing complexesby DNA affinity chromatography (34). In order to investigatethe formation of endogenous DNA-bound AML1/ETO-RBP-J ${kappa}$ complexes,RBP-J ${kappa}$ complexes were purified from Kasumi cells, which expressAML1/ETO (11). Complex purification was verified by EMSA andWestern blot analysis (Fig. 4A, lanes 7 to 9, and B, bottompanel, lanes 3 to 6). Western blot analyses further show thatAML1/ETO coelutes with RBP-J ${kappa}$ in fractions E2 and E3 (Fig. 4B,lanes 4 and 5). The presence of AML1/ETO within an endogenousRBP-J ${kappa}$ protein complex was additionally confirmed by immunoprecipitationexperiments with whole-cell lysates from Kasumi cells. For theprecipitation of AML1/ETO, an anti-ETO antibody was used. RBP-J ${kappa}$ could be coprecipitated with AML1/ETO, as shown by Western blotsprobed with an antibody against RBP-J ${kappa}$ (Fig. 4C, lane 2). Inaddition, RBP-J ${kappa}$ and AML1/ETO were also coimmunoprecipitatedby using an antibody directed against endogenous SHARP (Fig.4D, lanes 3 and 4). In order to investigate in vivo colocalizationexperiments with the fusion protein AML1/ETO and RBP-J ${kappa}$ , ChIPexperiments were performed using Kasumi cells. After precipitationwith specific antibodies, RBP-J ${kappa}$ and AML1/ETO were specificallyfound at the promoters of the Notch target Nrarp and cyclinD1 genes but not at the control (intron of the Hey1 gene) (Fig.4E).

View larger version (55K):
[in this window]
[in a new window]

FIG. 4. AML1/ETO is part of an endogenous RBP-J ${kappa}$ complex in Kasumi cells. (A) Purification of endogenous RBP-J ${kappa}$ complexes from Kasumi cells by DNA affinity chromatography. For purification, a DNA fragment containing 12 RBP-J ${kappa}$ -binding sites was biotinylated and immobilized on a streptavidin-Sepharose column. The column was incubated with whole-cell lysates from Kasumi cells. After incubation and washing, the DNA-bound RBP-J ${kappa}$ complexes were eluted with increasing concentrations of NaCl. (B) Western blot (WB) analysis of the lysate (lane 1), the first wash step (lane 2), and the eluted fractions (lanes 3 to 6) using antibodies against ETO ( ${alpha}$ ETO) and RBP-J ${kappa}$ ( ${alpha}$ RBP). AML1/ETO appears in the second and third elution steps, together with RBP-J ${kappa}$ (lanes 4 and 5). (C) RBP-J ${kappa}$ can be coimmunoprecipitated with AML1/ETO. Whole-cell lysates from Kasumi cells were incubated with an anti-ETO antibody overnight. The bound AML1/ETO complexes were immobilized on protein G-Sepharose beads. The cell lysates before (lane 1) and after precipitation (lane 2) were analyzed by Western blotting using an anti-RBP-J ${kappa}$ antibody. (D) RBP-J ${kappa}$ and AML1/ETO can be immunoprecipitated by using an antibody against SHARP. The cell lysates before (lanes 1 and 2) and after precipitation (lanes 3 and 4) were analyzed by using an anti-RBP-J ${kappa}$ antibody or an anti-ETO antibody, respectively. (E) ETO and RBP-J ${kappa}$ can be found associated at the promoter regions of the Notch target Nrarp and cyclin D1 genes in Kasumi cells. ChIP experiments were performed as described in Materials and Methods. Mean values and standard deviations (error bars) of four independent experiments are shown. As a control, an intron sequence of the Hey1 gene was used.

Taken together, these experiments demonstrate that AML1/ETOis a potential member of an endogenous DNA-bound RBP-J ${kappa}$ complexin Kasumi cells. The association between AML1/ETO and RBP-J ${kappa}$ is most probably mediated via SHARP, since we could not detecta direct interaction of AML1/ETO and RBP-J ${kappa}$ .

ETO, but not AML1/ETO, augments SHARP-mediated repression. ETO has previously been described as a transcriptional corepressor(reviewed in reference 16). In order to investigate whetherETO is also able to augment SHARP-mediated repression, we performedseveral functional assays. HeLa cells were cotransfected withexpression plasmids for Gal4-VP16-SHARP-RD, human ETO, or AML1/ETO,together with the Gal4-responsive reporter construct pFR-Luc.ETO enhanced the repression caused by Gal4-VP16-SHARP-RD ina dose-dependent manner up to fourfold (Fig. 5A). Surprisingly,the expression of AML1/ETO led to an up to twofold increasein promoter activity (Fig. 5A), suggesting that AML1/ETO interfereswith the repressional activity of SHARP. Several control experimentswere performed to probe the significance of these results (seeFig. S2 in the supplemental material). One, to exclude a possiblederegulation of the activator by ETO or AML1/ETO, protein expressionwas analyzed after transfection of HEK293 cells with Gal4-VP16-SHARP-RDalone or together with ETO or AML1/ETO by Western blotting (seeFig. S2A in the supplemental material). Two, HeLa cells werecotransfected with expression plasmids for Gal4-VP16-SHARP-RD,ETO (xl) or the ETO-related XETOR from Xenopus laevis (6), togetherwith the Gal4-responsive reporter construct pFR-Luc. ETO (xl),which showed a strong interaction with SHARP-RD (amino acids3477 to 3664) in GST pull-down experiments (see Fig. S2B, lane4, in the supplemental material), also enhanced the repressioncaused by Gal4-VP16-SHARP-RD in a dose-dependent manner (seeFig. S2C in the supplemental material). In contrast, XETOR,which failed to interact with SHARP (see Fig. S2B, lane 6, inthe supplemental material), had no effect on promoter activity(see Fig. S2C in the supplemental material).

View larger version (22K):
[in this window]
[in a new window]

FIG. 5. ETO, in contrast to AML1/ETO, acts as a corepressor for SHARP. (A) Human ETO increases, in a dose-dependent manner, the repression of promoter activity caused by SHARP-RD. In contrast, AML1/ETO increases the promoter activity. HeLa cells were transfected with the reporter construct pFR-Luc, the expression plasmid for the Gal4-VP16 fusion of SHARP-RD, and increasing amounts (100 ng and 150 ng) of the expression plasmids for ETO and AML1/ETO. (B) The repression caused by SHARP-RD and ETO is HDAC dependent. The reporter construct pFR-Luc was transfected alone or together with the expression plasmids for the Gal4-VP16 fusions and ETO into HeLa cells. The transfected cells were incubated for 6 h with TSA. The promoter activity was fully restored after the addition of TSA. Mean values and standard deviations (error bars) of at least four independent experiments are shown. rel., relative; –, absence of; +, presence of.

Previous studies have shown that ETO acts as an HDAC-dependentcorepressor (28). To determine whether the repressional effectof ETO and SHARP is mediated by HDAC activity, HeLa cells weretransfected with expression plasmids for Gal4-VP16 or Gal4-VP16-SHARP-RDand ETO, together with the Gal4-responsive reporter construct.Subsequently, the cells were treated with the HDAC inhibitortrichostatin A (TSA). The repression of the promoter activitycaused by Gal4-VP16-SHARP-RD and ETO was completely abolishedafter TSA treatment (Fig. 5B). GST pull-down assays showed thatcell-free synthesized HDAC1 directly interacts with GST-ETO.We also observed a direct interaction between HDAC1 and GST-AML1/ETOin GST pull-down assays (see Fig. S3 in the supplemental material).However, AML1/ETO did not act as a corepressor for SHARP.

ETO but not AML1/ETO represses RBP-VP16 mediated transcription. We have shown previously that RBP-J ${kappa}$ /Notch-IC interaction isnot compatible with RBP-J ${kappa}$ /SHARP interaction due to competitivebinding (32). The RBP-J ${kappa}$ /Notch-IC-recruited coactivator complexis different from the RBP-J ${kappa}$ /SHARP corepressor complex. To analyzethe effect of ETO and AML1/ETO on Notch-1-IC activated transcription,we performed luciferase assays with the artificial promoterconstruct pGA981/6 containing several RBP-J ${kappa}$ -binding sites. Thepromoter activity stimulated with Notch-1-IC was not changedby either ETO or AML1/ETO. In contrast, the cotransfection ofa SHARP construct containing only the RBP-J ${kappa}$ binding domain (aminoacids 2770 to 3127) resulted in a clear reduction of promoteractivity, most probably due to the displacement of the coactivatorcomplex and not to repression (Fig. 6A). To analyze the effectof ETO and AML1/ETO in an RBP-J ${kappa}$ /SHARP-dependent manner, thepromoter construct was activated by cotransfection with RBP-VP16(Fig. 6B), as shown previously (34). Promoter activity prestimulatedwith RBP-VP16 was reduced more than twofold by ETO, whereasAML1/ETO had no repressive effect on the promoter activity (Fig.6B). In addition, treatment of the cells with the HDAC inhibitorTSA almost fully restored the promoter activity (Fig. 6B).

View larger version (26K):
[in this window]
[in a new window]

FIG. 6. (A) ETO and AML1/ETO have no effect on the Notch-IC-recruited coactivator. The artificial reporter construct pGA981/6 was transfected into HeLa cells alone or together with a Notch-1-IC expression plasmid and an expression plasmid (100 ng) for ETO, AML1/ETO, or SHARP (amino acids 2779 to 3127). (B) ETO but not AML1/ETO acts as a corepressor for RBP-VP16-mediated transcription. The pGA981/6 reporter was transfected into HeLa cells alone or together with the RBP-VP16 expression plasmid and increasing amounts of expression plasmid (50 ng and 100 ng) for ETO and AML1/ETO. Where indicated, the HDAC inhibitor TSA (150 nM) was added to the cells 8 h prior to cell harvesting. Mean values and standard deviations (error bars) of at least three independent experiments are shown. rel., relative; –, absence of; +, presence of.

ETO but not AML1/ETO represses Hey1 and HES1 promoter activity. In humans, the HES1 and Hey1 genes had been identified as Notchtarget genes. In order to investigate the influence of ETO onthese two Notch targets, luciferase assays were performed byusing reporter constructs driven by either the HES1 or the Hey1promoter. Cotransfection of RBP-VP16, together with the ETOexpression plasmid, strongly reduced the promoter activity ina dose-dependent manner (Fig. 7A and B). Interestingly, cotransfectionwith AML1/ETO expression plasmid resulted in a slight activationof RBP-VP16-mediated transcriptional activity of the HES1 promoterconstruct (Fig. 7A), whereas AML1/ETO had no effect on the RBP-VP16-mediatedtranscriptional activity of the Hey1 reporter (Fig. 7B). Theexpression of the activator RBP-VP16 after the cotransfectionof ETO or AML1/ETO was again tested by Western blotting (seeFig. S4 in the supplemental material). After treatment of thecells with TSA, the promoter activity was almost fully restoredin all cases, suggesting that the ETO-mediated repression isindeed HDAC dependent (Fig. 7A and B).

View larger version (23K):
[in this window]
[in a new window]

FIG. 7. ETO, but not AML1/ETO, acts as a corepressor for a RBP-J ${kappa}$ -mediated transcription of HES1 (A) and Hey1 (B) genes. The reporter constructs were transfected into HeLa cells alone or together with the RBP-VP16 expression plasmid and increasing amounts of expression plasmid (50 ng and 100 ng) for ETO and AML1/ETO. Where indicated, the HDAC inhibitor TSA (150 nM) was added to the cells 8 h prior to cell harvesting. Mean values and standard deviations (error bars) of at least four independent experiments are shown. rel., relative; –, absence of; +, presence of.

Either knockdown of ETO1 or overexpression of AML1/ETO activates Notch target genes. In order to investigate the loss of function of ETO at endogenousNotch target genes, we performed knockdown experiments in apre-T-cell line derived from T-cell receptor beta knockout mice(Beko) that exclusively express ETO1 and not ETO2. Retroviralinfection with two independent ETO1 siRNAs led to an upregulationof the Notch target HES1 and Nrarp genes and to a very minorupregulation of the Hey1 gene (Fig. 8). To analyze the effectof AML1/ETO expression on endogenous Notch target genes, wetransfected HEK293 cells with expression plasmids for eitherAML1/ETO or the C-terminally truncated AML1/ETO(tr) that haspreviously been described (46) to be an even more potent oncogene.As a control, empty vector, Notch-IC, or RBP-VP16 was transfected.After mRNA isolation and cDNA synthesis, the expression of Hey2,p21^WAF1, and actin for normalization was studied by real-timePCR. AML1/ETO, like Notch-IC or RBP-VP16, stimulates transcriptionby up to sixfold in the case of Hey2 and two- to threefold inthe case of p21^WAF1 (Fig. 9).

View larger version (18K):
[in this window]
[in a new window]

FIG. 8. Knockdown of ETO1 activates the transcription of Notch target HES1 and Nrarp genes in pre-T cells. Two independent hairpins (ETO-1.1 and ETO-1.2) were used to infect a mouse pre-T-cell line. The expression of Notch target HES1 and Nrarp genes is upregulated, whereas the Hey1 gene level is only slightly affected. The values shown have been normalized with the expression of hypoxanthine phosphoribosyltransferase (HPRT). Mean values and standard deviations (error bars) of at least four independent measurements are shown. rel., relative.

View larger version (23K):
[in this window]
[in a new window]

FIG. 9. AML1/ETO and AML1/ETO(tr) activate transcription of the Notch target Hey2 and p21^Waf1 genes in HEK293 cells. Cells were transiently transfected with empty expression plasmid pcDNA3 or expression plasmid for AML1/ETO, AML1/ETO(tr), Notch-1-IC, or RBP-VP16. The mRNA levels of the Notch targets Hey2 and p21^Waf1 were determined by reverse transcription-PCR. As a control, the empty pcDNA3 vector was used. The values have been normalized with actin expression. Mean values and standard deviations (error bars) of at least four independent measurements are shown. rel., relative.

Specific knockdown of AML1/ETO leads to downregulation of Notch target genes. To analyze the effect of AML1/ETO on Notch target gene expressionin the leukemic Kasumi cell line expressing AML1/ETO due tothe t(8;21) translocation, we designed an siRNA that targetsa 25-nucleotide region spanning the fusion of AML1 and ETO.Kasumi cells were transfected with the pSIR-siRNA-internal ribosomeentry site-GFP vector expressing the specific AML1/ETO junctionhairpin. GFP-positive and GFP-negative cells were sorted byfluorescence-activated cell sorting and subsequently analyzedfor the expression of AML1, AML1/ETO, GAPDH (glyceraldehyde-3-phosphatedehydrogenase) for normalization, and several Notch target genes(Fig. 10). Specific downregulation of AML1/ETO mRNA, but notthat of AML1, was observed. The twofold knockdown effect wasalso described previously by two other groups (14, 19). In amanner similar to that described above, Notch target Nrarp,cyclin D1, and c-Myc genes were significantly downregulatedupon AML1/ETO knockdown (Fig. 10).

View larger version (16K):
[in this window]
[in a new window]

FIG. 10. Downregulation of the Notch target Nrarp, cyclin D1, and c-Myc genes after specific knockdown of AML1/ETO in Kasumi cells. Cells were transfected with a construct expressing a hairpin RNA directed against the AML1/ETO fusion region and GFP. After GFP-positive cells were sorted, relative (rel.) mRNA levels were determined by real-time PCR. The values have been normalized with the expression of GAPDH. Mean values and standard deviations (error bars) of four independent measurements are shown. rel., relative.

DISCUSSION

Top

DISCUSSION

RBP-J ${kappa}$ is the central player in the transcriptional regulationof Notch target genes and functions in both transcriptionalrepression and activation. Notch-IC enters the nucleus, bindsto RBP-J ${kappa}$ , and activates target genes. In the absence of Notch-IC,RBP-J ${kappa}$ recruits a corepressor complex that keeps Notch targetgenes inactive. Previously, we described SHARP as an RBP-J ${kappa}$ -interactingcorepressor (32). We could subsequently show that corepressorsCtIP and CtBP are recruited by RBP-J ${kappa}$ /SHARP to repress transcriptionof the Notch target gene Hey1 (34). Here, we have investigatedthe role of ETO and the leukemogenic fusion protein AML1/ETOin RBP-J ${kappa}$ /SHARP-mediated repression of Notch target genes andcould demonstrate that ETO, but not AML1/ETO, is able to augmentRBP-J ${kappa}$ /SHARP-mediated repression of Notch target genes.

The repression domain of SHARP functions as a platform for different corepressors. It has previously been shown that the SHARP repression domaincan interact with SMRT and N-CoR (37) as well as with CtIP/CtBP(34). In the present study, we show the functional interactionof SHARP and ETO. These observations suggest a redundancy inthe sense that different repressor complexes act at differentNotch target genes or in different cell types. Alternatively,the RBP-J ${kappa}$ /SHARP corepressor complexes might cross talk withother repressor complexes.

Mechanism of AML1/ETO-mediated disruption of repression. It has previously been described that AML1/ETO acts in a dominantmanner to inhibit AML1-mediated transcription (reviewed in reference7). However, there are reports which indicate that AML1/ETOcan be an activator regarding Bcl-2 (20) and enhance the expressionof p21^Waf1 (35) and HES1 (1). Our finding that ETO, but notAML1/ETO, can act in concert with RBP-J ${kappa}$ /SHARP to repress transcriptionat Notch target genes was surprising. Different potential scenariosmight explain our results at the molecular level. (i) The Runxdomain of AML1 is the binding domain of CBFβ, and thisheterodimer has been characterized extensively (47). The heterodimerof AML1/ETO and CBFβ could potentially activate Notch targetgenes. (ii) The Runx domain of AML has previously been describedto interact with other transcriptional activators, includingEts family factors, c-Jun/c-fos, and C-EBP family factors (reviewedin reference 36). Potentially, such an interactor causes transcriptionalactivation at Notch target genes. (iii) Alternatively, AML1/ETOand ETO localization in the nucleus could be affected in a waythat cannot be resolved by standard microscopic techniques.Both proteins have been found in the nucleus, but more carefulanalysis might reveal differences in localization. An alternativesplice variant of AML1/ETO that promotes leukemogenesis moreefficiently has previously been described (46). As shown inFig. 9, the truncated form of AML1/ETO, AML1/ETO(tr), upregulatesNotch target genes in a manner stronger than that of full-lengthAML1/ETO. The C-terminal region that is truncated contains NHR3and NHR4, which are also the binding sites for SMRT. It is possiblethat the lack of ETO repression in the AML1/ETO(tr) domain makesit an even better activator ("derepressor").

Upregulation of Jagged1 by AML1/ETO. It has previously been reported that the expression of AML1/ETOcauses the upregulation of the Notch ligand Jagged1 and therebyresults in the specific activation of Notch signaling throughthe Jagged1 ligand (1). Our results are in line with the upregulationof certain Notch target genes by AML1/ETO (see Fig. S5 in thesupplemental material). To test whether this upregulation ismediated by Notch processing due to ligand binding, we addedthe presenilin inhibitor N-[N-(3,5-difluorophenacetyl-L-alanyl)]-S-phenylglycinet-butyl ester (DAPT) to the cells expressing AML1/ETO or mNotch-1-IC- ${Delta}$ Eas a control. As expected, in mNotch-1-IC- ${Delta}$ E-expressing cells,DAPT downregulates the expression of luciferase from the HES1-specificreporter construct. In contrast, in AML1/ETO-expressing cells,DAPT has no effect on HES1 promoter activity (see Fig. S5 inthe supplemental material). Therefore, HES1 transactivationby AML1/ETO seems to be independent of Jagged1. These resultsargue against a positive autofeedback loop via Jagged1-mediatedNotch processing. Alternatively, we propose that AML1/ETO upregulatesNotch target genes by directly disrupting the normal corepressorfunction of SHARP/ETO.

Does derepression of Notch target genes by AML1/ETO contribute to leukemogenesis? The activation of Notch signaling favors the expansion of hematopoieticstem cells (reviewed in reference 27). These findings wouldbe in line with the observation that the leukemogenic fusionprotein AML1/ETO promotes the expression of certain Notch targetgenes. Retroviral transduction of hematopoietic stem cells ofAML1/ETO recapitulates many of the hematopoietic developmentalabnormalities seen in humans, but animals do not develop leukemiafor several months (8). This observation suggests that a principalcontribution of AML1/ETO to AML is to maintain the undifferentiatedstate or even expand these progenitor cells. The activationof Notch target genes might be crucial in this respect. We suggestthat endogenous ETO is a novel corepressor to keep Notch targetgene expression silent. The leukemogenic fusion protein AML1/ETOcan disrupt the repressive ETO function and activate certainNotch target genes. This in turn might favor the expansion ofhematopoietic progenitor cells and possibly contribute to leukemogenesis.

In summary, our results indicate that corepressor ETO is a novelcomponent of the RBP-J ${kappa}$ /SHARP corepressor complex and that ETO,but not AML1/ETO, augments repression at Notch target genes.It will be interesting to further investigate the significanceof the disruption of the repressive function ETO by AML1/ETOin myeloid leukemia.

ACKNOWLEDGMENTS

We thank J. Lausen, D. van Essen, M. Gessler, and Ying Cao forproviding us with plasmids and J. Kisielow for the pre-T-cellline Beko. We thank M. Krötschel, E. Rüber, R. Rittelmann,and S. Schirmer for excellent technical assistance.

This study was supported by the Deutsche ForschungsgemeinschaftEmmy-Noether fellowship (BO-1639/3-2) to T.B., DFG grants Wi-1990/2-1to J.W. and SFB497/B9 and SFB518/A18 to F.O., and by funds fromthe Max Planck Society (to T.B.).

FOOTNOTES

* Corresponding author. Mailing address for Tilman Borggrefe: Department of Cellular and Molecular Immunology, Max Planck Institute of Immunobiology, Stübeweg 51, 79108 Freiburg, Germany. Phone: 49-761-5108-715. Fax: 49-761-5108-799. E-mail: borggrefe{at}immunbio.mpg.de. Mailing address for Franz Oswald: Department of Internal Medicine I, University of Ulm, Robert-Koch-Str. 8, 89081 Ulm, Germany. Phone: 49-731-500-44544. Fax: 49-731-500-44502. E-mail: franz.oswald{at}uni-ulm.de

Published ahead of print on 10 March 2008.

Supplemental material for this article may be found at http://mcb.asm.org/.

These authors made equal contributions.

REFERENCES

Top