Ets-2 Repressor Factor Silences Extrasynaptic Utrophin by N-Box mediated Repression in Skeletal Muscle

doi:10.1091/mbc.E06-12-1069

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Originally published as MBC in Press, 10.1091/mbc.E06-12-1069 on May 16, 2007

Vol. 18, Issue 8, 2864-2872, August 2007

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Ets-2 Repressor Factor Silences Extrasynaptic Utrophin by N-Box–mediated Repression in Skeletal Muscle

Kelly J. Perkins^*^,, Utpal Basu^*, Murat T. Budak^*, Caroline Ketterer^*, Santhosh M. Baby^*, Olga Lozynska^*, John A. Lunde, Bernard J. Jasmin, Neal A. Rubinstein^*, and Tejvir S. Khurana^*

*Department of Physiology and Pennsylvania Muscle Institute, University of Pennsylvania School of Medicine, Philadelphia, PA 19104-6085; and Faculty of Medicine, University of Ottawa, Ottawa, Ontario K1H 8M5, Canada

Submitted December 4, 2006; Revised May 4, 2007; Accepted May 7, 2007
Monitoring Editor: William Tansey

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Utrophin is the autosomal homologue of dystrophin, the proteinproduct of the Duchenne's muscular dystrophy (DMD) locus. Utrophinexpression is temporally and spatially regulated being developmentallydown-regulated perinatally and enriched at neuromuscular junctions(NMJs) in adult muscle. Synaptic localization of utrophin occursin part by heregulin-mediated extracellular signal-regulatedkinase (ERK)-phosphorylation, leading to binding of GABP ${alpha}$ / $beta$ tothe N-box/EBS and activation of the major utrophin promoter-Aexpressed in myofibers. However, molecular mechanisms contributingto concurrent extrasynaptic silencing that must occur to achieveNMJ localization are unknown. We demonstrate that the Ets-2repressor factor (ERF) represses extrasynaptic utrophin-A inmuscle. Gel shift and chromatin immunoprecipitation studiesdemonstrated physical association of ERF with the utrophin-Apromoter N-box/EBS site. ERF overexpression repressed utrophin-Apromoter activity; conversely, small interfering RNA-mediatedERF knockdown enhanced promoter activity as well as endogenousutrophin mRNA levels in cultured muscle cells in vitro. Laser-capturemicroscopy of tibialis anterior NMJ and extrasynaptic transcriptomesand gene transfer studies provide spatial and direct evidence,respectively, for ERF-mediated utrophin repression in vivo.Together, these studies suggest "repressing repressors" as apotential strategy for achieving utrophin up-regulation in DMD,and they provide a model for utrophin-A regulation in muscle.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Duchenne's muscular dystrophy (DMD) is a fatal neuromusculardisease caused by gene mutations leading to qualitative or quantitativedisturbances in dystrophin expression (Hoffman et al., 1987).Dystrophin-related protein or utrophin is considered the autosomalhomologue of dystrophin, because it shares extensive sequencehomology as well as its size and abundance in muscle (Love etal., 1989; Khurana et al., 1990; Tinsley et al., 1992). Utrophinand dystrophin also share functional properties such as theability to associate with the dystroglycan complex and bindF-actin (Matsumura et al., 1992; Winder and Kendrick, 1995;Rybakova et al., 2002). Direct evidence for the ability of utrophinto functionally substitute comes from experiments demonstratingthat utrophin overexpression driven either by transgenic means(Tinsley et al., 1996; Rafael et al., 1998; Tinsley et al.,1998; Fisher et al., 2001) or viral vectors (Gilbert et al.,1999; Wakefield et al., 2000; Cerletti et al., 2003) can rescuedystrophin-deficient muscle. Despite these functional similarities,dystrophin and utrophin exhibit distinct localization in normaladult tissues. Perinatally, utrophin is expressed throughoutthe sarcolemma, however, its expression declines as that ofdystrophin increases (Khurana et al., 1991; Clerk et al., 1993),leading to its spatially restricted expression at neuromuscularand myotendinous junctions (NMJs and MTJs, respectively) ofadult myofibers. These features and relevance toward a therapyfor DMD provide a powerful impetus for better understandingtranscriptional control of utrophin expression in myofibers(Jasmin et al., 2002; Khurana and Davies, 2003; Nowak and Davies,2004).

Although full-length utrophin protein can be generated usingindependently regulated A (Dennis et al., 1996) and B (Burtonet al., 1999) promoters, myofiber utrophin expression is chieflycontrolled via the utrophin-A promoter (Weir et al., 2002; Chakkalakalet al., 2003), and it is thus the subject of this investigation.Spatial and temporal expression of utrophin-A at the NMJ parallelsthat of nicotinic acetylcholine receptor (nACHR) subunits. Indeed,these genes share some features of transcriptional control.For example, the nACHR ${varepsilon}$ subunit and utrophin-A promoter N-boxplay a critical role in regulating expression levels and moreimportantly in restricting expression to the NMJ (Schaefferet al., 2001). We and others (Gramolini et al., 1999a; Khuranaet al., 1999) have shown that the nerve-derived growth factorheregulin (HRG) causes a N-box–mediated increase in utrophin-Apromoter activity via extracellular signal-regulated kinase-dependentactivation of the Ets-related transcription factor complex GABP ${alpha}$ / $beta$ ,in a manner similar to that noted in the nACHR ${delta}$ and nACHR ${varepsilon}$ subunitpromoters (Falls et al., 1993; Koike et al., 1995; Sapru etal., 1998; Schaeffer et al., 1998). Additionally, SP1 (Galvagniet al., 2001; Gyrd-Hansen et al., 2002), NFATc1/calcineurin(Chakkalakal et al., 2003; Chakkalakal et al., 2004), and myogenicfactors (Gramolini and Jasmin, 1999; Perkins et al., 2001) canalso activate the utrophin-A promoter. Recently, the 5'-untranslatedregion of utrophin-A promoter has been shown to be importantfor regulation of utrophin protein levels during regenerationas well (Miura et al., 2005). Indeed, several of these moleculesor mechanisms are currently being investigated for developmentof utrophin up-regulation-based therapeutics for DMD (Chaubourtet al., 1999; Krag et al., 2004; St-Pierre et al., 2004; Segalatet al., 2005).

However, equally important mechanisms controlling concurrentextrasynaptic down-regulation or repression of utrophin-A inmyofibers that must occur to achieve expression at the NMJ ratherthan generalized expression throughout the sarcolemma remainunaddressed. Mechanistic clues arise from studies illustratingthat restriction of neuronal sodium channel expression to thenervous system is partly due to RE-1 silencing transcriptionfactor/neuronal-restricted silencing factor binding to a repressorelement (Andres et al., 1999; Ballas et al., 2001; Lunyak etal., 2002). Additionally an N-box–mediated silencing mechanismhas been suggested for nACHR subunit expression in extrasynapticregions of muscle (Koike et al., 1995). In silico analysis ofthe human and murine utrophin-A promoter sequences suggest Ets-2repressor factor (ERF) as a candidate molecule for N-box–mediatedextrasynaptic repression of the utrophin-A promoter (Sgouraset al., 1995). ERF is a novel member of the ets family and encodesa ubiquitously expressed 548-amino acid phospho-protein identifiedthrough its ability to repress the Ets-2 promoter via EBS binding(Sgouras et al., 1995; Le Gallic et al., 1999). ERF activityis regulated in part, by ERK-dependent changes in its phosphorylationstatus and subcellular localization due to nuclear shuttling,with CRM1 suggested to have a role in ERF export (Le Gallicet al., 2004). Here, we use an array of in vitro and in vivomethodologies to delineate the role of ERF in the regulationof the utrophin-A promoter.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Constructs
The pPUBF utrophin promoter luciferase reporter construct contains1.3-kb of human utrophin promoter-A sequence (Dennis et al.,1996), and it was a kind gift from Prof. Kay Davies (OxfordUniversity). The pPUBF ${Delta}$ N-box is a pPUBF derivative with a deletedN-box/EBS sequence, and it has been previously described byour laboratory (Khurana et al., 1999). Expression vectors containinghuman GABP ${alpha}$ and - $beta$ 1 subunits used were GABP ${alpha}$ and GABP $beta$ (Rosmarinet al., 1995), and they were kindly gifted by Prof. Alan Rosmarin(Brown University). Expression vectors containing human ERFcDNA used were pSG5-ERF and GFP-ERF (Sgouras et al., 1995; LeGallic et al., 1999), and they were kindly gifted by Prof. GeorgeMavrothalassitis (IMBB, Greece).

Gel Shift Assay
Double-stranded probes encompassing the EBS and N-box of thehuman utrophin-A promoter (5'-GCTGATCTTCCGGAACAAAGTTGCT-3';N-box underlined; EBS bold) or probes containing a mutated N-box/EBSsite (5'-GCTGATCTTCCATCTACAAGTTGCT-3') were end labeled with[ ${gamma}$ -³²P]ATP by using polynucleotide kinase. Unlabeled probes (10-and 100-fold excess) were used in cold competitor assays asoutlined in Figure 1B. Recombinant human ERF (rhERF) was producedusing a coupled in vitro transcription/translation system (Promega,Madison, WI), by using 0.5 µg (GFP)-ERF construct andunlabeled methionine. Additionally, we used nuclear extractsfrom C2C12 cell line (Active Motif, Carlsbad, CA). Gel shiftanalysis was performed using the Gel Shift Assay system (Promega).For supershifts, 5 µl of ERF-specific rabbit polyclonalantibody (S17C), and as controls, a nonspecific polyclonal antibodyagainst the transcription factor Twist (Santa Cruz Biotechnology,Santa Cruz, CA), were added to the reaction mix for 1 h at roomtemperature before probe addition. Protein–DNA complexeswere resolved on 4% polyacrylamide gels by using 0.25x Tris-glycinebuffer at 200 V for 2 h. Gels were dried and autoradiographedon a Typhoon 8600 Imager (GE Healthcare, Little Chalfont, Buckinghamshire,United Kingdom).

Semiquantitative Reverse Transcription-Polymerase Chain Reaction (RT-PCR)
RT-PCR was performed on RNA obtained from $~$ 100 mg of freshlydissected dystrophin-deficient (mdx) hindlimb muscle from differentdevelopmental stages, as described previously (Khurana et al.,1999). Murine ERF and GABP ${alpha}$ primers were designed to amplifya 490-base pair fragment of ERF spanning exons 1–4 (ERF1F,5'-GATTGGCCTACAAACCGGAGTCATCC-3') and ERF2R, 5'-GTC GGGCAACCACAGGAGAGAAGAG-3')and a 409-bp fragment of GABP ${alpha}$ spanning exons 8–10 (GABP ${alpha}$ 2F,5'-CAGCTAAAGTGCAACGGTCCCCAAG-3' and GABP ${alpha}$ 1R, 5'-CCGTGCCAGTTTCTTCTGTTCACACTC-3').Primers used for MyoD were M_MyoD_1483F (5'-CTCCACATCCTTTTGTTTGT-3')and M_MyoD_1825R (5'-AGCGTCTTTATTTCCAACAC-3') and for Myogeninwere M_Myogenin_924F (5'-CAATACACAAAGCACTGGAA-3') and M_Myogenin_1222R(5'-TCTGAGGAGAGAAAGATGGA-3'). Utrophin and glyceraldehyde-3-phosphatedehydrogenase (GAPDH) primers were as described previously (Khuranaet al., 1999). PCR products were resolved on 4% acrylamide gels,dried, and radioactively incorporated products quantified usinga Typhoon 8600 Imager and ImageQuant IQ Tools version 2.2 (GEHealthcare).

Tissue Culture and Transfection
Murine C2C12 muscle cells and Drosophila S2 embryonic cellswere maintained and transfected as described previously (Gyrd-Hansenet al., 2002). For cotransfection of human GABP ${alpha}$ , GABP $beta$ , and pSG5-ERFexpression vectors, 1 µg of vector(s) and 1 ng of Renillacontrol plasmid (pRL-TK; Promega) were used. The mitogen-activatedprotein kinase kinase (MEK) inhibitor UO126 (10 µM; Promega)was added concurrent with transfection to block Drosophila (GobertGosse et al., 2005) and mammalian MEK activity. Cells were allowedto express fusion genes for 12–24 h before analysis ofcell extracts for luciferase activity by using the Dual LuciferaseAssay kit (Promega) with a 20/20 luminometer (Turner Designs,Sunnyvale, CA). All assays were performed in triplicate withthe transfection/assay process repeated using separate culturesfor particular experiments as outlined in the figure legends.

MEK-dependent translocation of ERF from nucleus to cytoplasmwas studied using C2C12 muscle cells that were incubated withMEK inhibitor U0126 for different times and analyzed using immunofluorescenceof cells and immunoblotting of subcellular fractions as describedpreviously for Ref1 cells (Le Gallic et al., 1999, 2004). Forimmunofluorescent analysis, cells were fixed with ice-cold methanolfor 10 min, incubated with anti-ERF antibodies (Santa Cruz Biotechnology),and detected using Alexa Fluor 546 donkey anti-goat secondaryantibodies (Invitrogen, Carlsbad, CA). Images were acquiredusing a Radiance 2000 confocal laser imaging system (Bio-Rad,Hercules, CA). Nuclear and cytoplasmic fractions for immunoblottingwere obtained by lysing the cells with 35 strokes in a glassDounce homogenizer (pestle B) in buffer A (10 mM Tris-HCl, pH7.5, 300 mM sucrose, and 1 mM EDTA). Nuclei were pelleted at2000 x g for 5 min and washed with buffer B (10 mM HEPES, 10mM NaCl, 1 mM KH₂PO₄, 5 mM NaHCO₃, 1 mM CaCl₂, 0.5 mM MgCl₂,and 0.1% Nonidet P-40). All buffers were supplemented with 1mM orthovanadate and protease inhibitor complete (Roche Diagnostics,Basel, Switzerland). To control for fractionation of nuclearand cytoplasmic compartments, aliquots of each of the fractionswere monitored using fluorescent microscopy and DNA bindingdyes. To control for loading equivalent amounts of proteins,the concentration of proteins was measured using a Bradfordassay (Bio-Rad), and equal concentration (50 µg) of totalprotein from cytoplasmic and nuclear fractions were loaded andresolved using 3–8% Tris-acetate gradient SDS-polyacrylamidegel electrophoresis, electrotransferred onto polyvinylidenedifluoride membrane (Immobilon-P; Millipore, Billerica, MA),and membranes were probed using anti-ERF antibodies (Santa CruzBiotechnology). Blots were washed thoroughly, incubated withhorseradish peroxidase-conjugated donkey anti-goat secondaryantibodies (Promega), and enhanced chemiluminescence was performedas described by manufacturer (Pierce Chemical, Rockford, IL),by using X-Omat Blue XB-1 films (Eastman Kodak, Rochester, NY).

RNA Interference (Small Interfering RNA) Studies
Duplexed stealth RNA oligomers to the murine ERF sequence weredesigned using the BLOCK-iT RNA interference system (Invitrogen).Proliferating C2C12 cells (50% confluent) were transfected usingLipofectAMINE 2000 (Invitrogen) with 25 pmol each of ERF-292(5'-GGUUCACCUACAAG UUCAACUUCAA-3'), ERF-326 (5'-GCUGGUCAAUUACCCUUUCAUCGAU-3'),ERF-937 (5'-CCCACACCCAAAGCGUCUACAACUA-3'), and ERF-1268 (5'-GAUUAAGGUGGAGCCCAUCUCAGAA-3') or 100 pmol of an unrelated, scrambled control"egg" oligomer (5'-GCUUACUC AUCCAUGCAUCGGUAUG-3'). Transcriptlevels of utrophin, GAPDH, and ERF postoligomer addition weredetermined using semiquantitative RT-PCR. Analysis of ERF knockdowneffects on utrophin promoter activity used 1 µg of pPUBFconstruct and transfection of oligomers after 24 h. Cells wereincubated an additional 24 h before assaying for luciferaseactivity.

Chromatin Immunoprecipitation (ChIP)
ChIP was performed with goat polyclonal anti-ERF antibodies(Santa Cruz Biotechnology) according to the manufacturer's protocol(Upstate Biotechnology, Lake Placid, NY). Briefly, cells fromone 100-mm plate were treated with or without 2 nM heregulinfor 15 min after overnight serum starvation, and they were cross-linkedwith 0.37% final concentration of formaldehyde. For U0126 treatment,cells were grown in presence of serum and treated with 10 µMU0126 for 15 min. Cells were washed twice with ice-cold phosphate-bufferedsaline (PBS). Cell pellets were lysed in 200 µl of lysisbuffer and sonicated. Cell lysate was diluted 10-fold in ChIPdilution buffer and precleared with 120 µl of proteinA-agarose and 120 µl of protein G-agarose. The preclearedset was incubated with or without antibody at 4°C overnightwith constant rotation. The antibody–chromatin complexwas then collected with 60 µl of protein A-agarose and60 µl of protein G-agarose, incubating 1 h at 4°Cwith constant rotation. The agarose beads were washed with washbuffers, and finally, chromatin was eluted with 500 µlof elution buffer (0.1 M NaHCO₃ and 1% SDS) at room temperature.Beads were reverse cross-linked at 65°C overnight with 20µl of 5 M NaCl. One percent of input reserved before immunoprecipitationwas reverse cross-linked in parallel. All solutions were supplementedwith protease inhibitor complete (Roche Diagnostics), 1 mM Na₃VO₄and 1 mM NaF. DNA was extracted with PCR purification kit (QIAGEN,Valencia, CA). Presence of utrophin-A promoter was detectedin different sets by PCR in the presence of [ ${alpha}$ -³²P]dCTP withprimers 5'-CCCAAACTCAACAACCTCAGTAAAC-3' and 5'-CAAATTGTCCGAAAATGTGTGTCA-3'designed to amplify 151 bp of utrophin-A promoter (NCBI accessionno. X95524). Primers did not amplify products without appropriatetemplates. The products were separated using 12% acrylamidegel, and they were imaged using a Typhoon 8600 (GE Healthcare).

Laser Capture Microdissection (LCM) and Quantitative (q)PCR
Microscopy was performed using a PALM laser capture microscopewith sections of adult rat tibialis anterior (TA) muscle (200–300µm² and 10 µm in thickness) by using methods similarto those used for regional expression profiling of muscle (Budaket al., 2004; Nazarian et al., 2005). Extracted total RNA (yieldtypically between 50 and 150 ng) was used for one cycle linearamplification by using the Affymetrix two-cycle labeling kit(Affymetrix, Santa Clara, CA). Subsequently, amplified RNA (aRNA;yield typically 1000–5000 ng) was converted to cDNA byusing an Invitrogen SuperScript RT kit and used as a templatefor qPCR. Taqman qPCR cholinergic receptor, nicotinic, ${alpha}$ polypeptide1 (Chrna1) (assay ID Rn00577938_m1), Utrn (utrophin) (assayID Rn00565137_m1, murine Ets-2 repressor factor (Erf) (mouse,assay ID Mm00468761_m1) and $beta$ actin primers (part 4352931E; AppliedBiosystems, Foster City, CA). Rat v-ets erythroblastosis virusE26 oncogene homologue 1 (Ets1) (forward, 5'-TTGTGTGTGACCCGGAAGC-3'and reverse, 5'-GCTGATTATCCGGAAAGGCC-3') primers were designedby primer expressed software version 2 for SYBR Green chemistryqPCR. An ABI 7500 qPCR machine (Applied Biosystems) was usedfor Taqman qPCR and ABI 7900HT qPCR machine (Applied Biosystems)was used for SYBR Green chemistry. cDNA (RNA) template (an aRNAequivalent of 3–5 ng/well cDNA used) of same animal wasrun in duplicate on the plate, and results were analyzed usingthe delta count method for relative gene expression analysisby using ABI SDS software version 1.3.1 (Applied Biosystems).

Direct Gene Transfer
All animal care and experimental procedures were performed inaccordance with the guidelines established by the Canadian Councilof Animal Care. These procedures were approved by the Universityof Ottawa Animal Care and Use Committee. Three- to 4-wk-oldC57BL/6 mice were anesthetized, and anterior portions of bothlower hindlimbs were shaved and disinfected. The underlyingTA muscles were then directly injected with 25 µl of DNAsolution as described previously (Gramolini et al., 1997; Chakkalakalet al., 2003). The DNA solution contained equal amounts of the1.3-kb human utrophin-A promoter-reporter (LacZ) construct (seeGramolini et al., 1997; Chakkalakal et al., 2003), the pPUBF ${Delta}$ N-boxconstruct (luciferase), a constitutively expressed chloramphenicolacetyl transferase (CAT) plasmid (to control for transductionefficiency), and either the ERF expression plasmid or its control(pSG5). Plasmid DNA was prepared using the Mega-Prep kit (QIAGEN,Mississauga, Ontario, Canada). DNA pellets were resuspendedin sterile PBS at a final concentration of 1–2 µg/µl.Five days postinjection, TA muscles were quickly excised, immediatelyfrozen in liquid nitrogen, and stored at –80 C until processedfor RT-PCR analysis. Total RNA was extracted by using TriPure(Roche Diagnostics, Indianapolis, IN) as recommended by themanufacturer. Quantitative RT-PCR was performed to determinethe relative abundance of LacZ, luciferase, and CAT transcripts.Before RT-PCR, samples were digested using DNase1 to eliminatepossible plasmid contamination (Gramolini et al., 2001). RT-PCRassays were performed using previously described protocols andprimers (Gramolini et al., 1999b, 2001; Chakkalakal et al.,2003). Cycle numbers varied depending on the primers used andthey were all within the linear range of amplification. In allassays, negative controls consisted of RT mixtures in whichtotal RNA was replaced with RNase-free water. PCR products werefirst visualized on 1.5% agarose gels containing ethidium bromide.Labeling intensity of the PCR products that is linearly relatedto the abundance of cDNAs was then quantified using DigitalScience 1D Image Analysis software (Eastman Kodak). Values werestandardized relative to the amount of CAT present in the samesample. The Student's t tests were used to analyze the data.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ERF Can Physically Associate with the Utrophin-A N-Box/EBS Site
To determine whether the utrophin-A promoter N-box/EBS sequenceis recognized by ERF, a double-stranded probe spanning the region(Figure 1A) was incubated with recombinant ERF (Sgouras et al.,1995) for gel shift assays. The protein–DNA complex couldbe competed with excess unlabeled N-box/EBS probe and supershiftedusing ERF-specific antibodies (Figure 1B). The protein–DNAcomplex could not be competed using a probe containing mutationsin the N-box/EBS. The complex was not supershifted using anirrelevant antibody. Additionally, a mutant probe was not retardedwhen incubated with ERF (Figure 1B). To demonstrate the existenceof ERF and show its ability to form the complex in the contextof muscle, we performed the gel shift and supershift by usingnuclear extracts obtained from C2C12 muscle cell lines. As shownin Figure 1B, a protein–DNA complex was formed that wasable to retard probe migration and able to be competed withexcess unlabeled probe as well as supershifted using ERF-specificantibodies in muscle cell lines, suggesting the relevance ofthis mechanism for muscle in vivo.

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Figure 1. ERF binds to the utrophin-A promoter N-box/EBS element. (A) Sequence of the human utrophin-A promoter probes containing the N-box/EBS motif used in gel shifts. The N-box is in bold italics; the EBS is in a white box. Mutant refers to the gel shift probe used that contains a mutant N-box/EBS site. (B) The N-box/EBS site in the human utrophin A promoter binds ERF. rhERF was in vitro synthesized and 0.5–10 µl (0.5–10; lanes 2–5) was incubated with the labeled oligonucleotide probe. Five microliters each of C2C12 extract was used for analysis of endogenous ERF in lanes 17–22. Formation of a single specific DNA–protein complex (gray arrow) was observed with rhERF (lanes 2–5), which could be specifically competed away with 10- and 100-fold excess of wild-type cold competitor oligonucleotide (lanes 6 and 7) but not the mutant probe (lanes 8 and 9). rhERF did not bind a double-stranded probe of the same region with a mutated N-box/EBS site (lanes 10–12). The black arrow indicates ERF–DNA complex supershifted in the presence of 5 µl of ERF-specific antibodies (lane 14) but not in the presence of a nonspecific antibody against the transcription factor Twist (lane 13). White arrows represent free radiolabeled probe. Wt, wild-type probe; mt, N-box/EBS mutant probe; [ERF], amount of rhERF protein in microliters; c, comp, unlabeled N-box/EBS oligonucleotide; ${alpha}$ ERF, ERF S17C rabbit polyclonal antibody.

Having demonstrated the ability of ERF to associate with theN-box/EBS site of the utrophin-A promoter using gel shift assays,we asked whether the ERK-dependent nuclear shuttling mechanismspreviously characterized in Ref-1 cells (Le Gallic et al., 2004

)are functional in C2C12 muscle cell lines. To test this, weperformed subcellular fractionation experiments to determinethe levels of ERF in the nuclear and cytoplasmic fractions ofC2C12 muscle cell lines after incubation with U0126, an inhibitorfor MEK, the upstream kinase for ERK1/2 at different times.As shown in Figure 2Ai, incubation with U0126 led to increasedERF levels in the nuclear compared with cytoplasmic fractions.Next we used anti-ERF antibodies for indirect immunofluorescentconfocal microscopy to independently validate the MEK-dependentnuclear shuttling by visualizing changes in subcellular localizationof ERF in C2C12 cells when incubated with U0126. As shown inFigure 2Aii, incubation with U0126 caused ERF to preferentiallylocalize in the nucleus. To demonstrate the effect of ERF onutrophin-A promoter activity, we used the pPUBF utrophin-A luciferasereporter construct containing the entire human utrophin promoter(Dennis et al., 1996

), as well as the pUBF ${Delta}$ N-box reporter constructthat contains a deletion mutation of the N-box region (Khuranaet al., 1999

) (Figure 2Bi). Drosophila S2 cells were cotransfectedwith pPUBF and 1) expression constructs encoding GABP ${alpha}$ / $beta$ (Rosmarinet al., 1995

) as a positive control or 2) ERF expression vectorpSG5-ERF. In agreement with previous studies (Khurana et al.,1999

; Gyrd-Hansen et al., 2002

), GABP ${alpha}$ / $beta$ trans-activated the utrophinA promoter fourfold (407 ± 39.2%) (Figure 2Bii). In contrast,ERF trans-repressed the promoter by $~$ 88% (12.3 ± 2.2%).Use of the MEK inhibitor U0126 and the subsequent nuclear exportof ERF also resulted in an approximately threefold decreasein promoter activity (32.1 ± 9.3%). Utrophin promoterreporter assays were also performed using cotransfection ofERF and GABP ${alpha}$ / $beta$ expression constructs together in Drosophila S2cells (Figure 2B). To determine whether the N-box was requiredfor ERF-mediated repression, we transfected cells using thepUBF ${Delta}$ N-box construct. As shown in Figure 2Bii, ERF was unableto repress the mutant utrophin promoter lacking the N-box motif.Additionally, immunoblotting by using anti-ERF and anti-GABPantibodies was performed on cells that had been transfectedwith the ERF and GABP constructs, respectively, to verify thatthe expression constructs were functional (Figure 2Biii). Together,these assays demonstrated that 1) ERF-mediated trans-repressioncould be successfully competed by GABP ${alpha}$ / $beta$ -mediated promoter activationand 2) that the N-box motif is required for ERF-mediated trans-repressionof the utrophin promoter.

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Figure 2. The human utrophin-A promoter is trans-repressed by ERF overexpression and MEK inhibition, which may be alleviated by GABP ${alpha}$ / $beta$ . (A) Changes in subcellular fractions and subcellular localization of ERF protein in C2C12 cells caused by inhibition of MEK by using U1026. Nuclear shuttling of ERF noted over a 30-min treatment period as demonstrated by i) immunoblotting or ii) immunofluorescence by using anti-ERF antibodies, as described in Materials and Methods. Bar, 25 µm. (B) The human utrophin-A promoter is trans-repressed by ERF overexpression and MEK inhibition, which may be alleviated by GABP ${alpha}$ / $beta$ . (i) The 1.3-kb human utrophin-A promoter-luciferase construct pPUBF showing location of the N-box/EBS according to X95523. The pPUBF ${Delta}$ N-box construct has a deletion that removes the N-box/EBS. (ii) pPUBF or pPUBF ${Delta}$ N-box derived firefly luciferase activities were normalized to pRL-TK-derived Renilla luciferase activity and expressed as a percentage of normalized luciferase activity (black column). Utrophin promoter-reporter constructs and a transfection control pRL-TK vector were cotransfected into S2 cells along with equimolar combinations of the following: GABP ${alpha}$ / $beta$ expression vectors (GABP, gray columns), ERF expression vector pSG5-ERF (ERF, white columns), GABP ${alpha}$ / $beta$ and ERF vectors (light gray column), or a 10 µM final concentration of MEK inhibitor UO126 (white column), and luciferase activity was assayed after a 24-h incubation. GABP ${alpha}$ / $beta$ trans-activated the utrophin promoter construct almost fourfold (gray column), whereas decreases to 12 and 33% of normalized promoter activity was noted with ERF overexpression and MEK inhibition, respectively. However, trans-repression by ERF was completely competed by GABP ${alpha}$ / $beta$ trans-activation (light gray column). No difference in pPUBF ${Delta}$ N-box reporter activity was observed upon the addition of ERF (96%). Luciferase values are the means of triplicate wells in nine separate experiments (n = 27) for pPUBF and ERF and in three separate experiments (n = 9) for MEK inhibition and GABP ${alpha}$ / $beta$ . Error bars are SEM. (iii) Immunoblot controls showing that transfection of GABP and ERF expression vectors causes an increase in protein levels in transfected C2C12 cells.

ERF Knockdown Enhances Endogenous Utrophin mRNA Levels and Utrophin-A Promoter Activity
Because ERF is able to bind and repress promoter activity, wesought to delineate the effect of siRNA-mediated silencing ofERF on 1) endogenous utrophin mRNA levels and 2) utrophin-Apromoter activity. To ensure selective knockdown, four siRNAoligomers corresponding to regions of ERF outside the conservedN-box/EBS binding domain with no homology to other known genewere transfected into C2C12 muscle cells, and semiquantitativeRT-PCR was performed after 24 h. ERF siRNA decreased endogenousERF levels to 2%, and it enhanced endogenous utrophin levels(1.4-fold) compared with an unrelated scrambled oligomer control(egg), after adjustment to GAPDH levels (Figure 3Ai). We postulatedthe increase in utrophin mRNA was due to increased promoteractivity as a result of decreased ERF levels; therefore, pPUBFwas transfected 24 h postoligomer addition, and C2C12 cellswere assayed for luciferase activity after an additional 24-hperiod (Figure 3Bii). In concordance with our hypothesis, atwofold elevation of promoter activity (199.1 ± 24%)was observed for ERF oligomers in comparison with the egg control.Additional transfection experiments were performed to addresswhether siRNA-mediated silencing of ERF altered the programof myogenic differentiation in the cultured myotubes and hencesecondarily effected utrophin expression via altered expressionof myogenic factors (Gramolini and Jasmin, 1999

; Perkins etal., 2001

). As shown in Figure 3Aiii, no alterations in expressionlevels of the myogenic factors MyoD and myogenin were detectedusing semiquantitative RT-PCR after transfecting with ERF siRNAoligomers or scrambled egg control, making it highly unlikelythat the alterations of utrophin promoter activity were dueto changes in expression of myogenic factors. Rather, the increasein utrophin promoter activity noted in Figure 3A was indeeda direct result of decreased ERF levels due to a siRNA-mediatedmechanism, as postulated.

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Figure 3. Inhibition of ERF gene expression enhances utrophin mRNA levels and utrophin-A promoter activity in C2C12 cells. (Ai) Semiquantitative RT-PCR of ERF, utrophin, and GAPDH transcript levels in murine C2C12 cells after treatment with either 100 pmol (left lane) of an unrelated, scrambled control egg oligomer, or 25 nmol each of four siRNA complementary to ERF. ERF siRNA oligomers caused a specific decrease in ERF transcript to $~$ 2% and an $~$ 1.4-fold increase in utrophin mRNA after adjustment to GAPDH levels. (ii) ERF knockdown causes an increase in utrophin promoter activity. The pPUBF utrophin promoter-luciferase construct was transfected into C2C12 cells 24 h after either egg or ERF siRNA oligomer transfection, and luciferase activity was assayed after an additional 24-h incubation. An approximate twofold elevation of utrophin promoter activity in C2C12 cells was observed with the ERF oligomer mix (1.99 ± 0.24) in comparison with the egg scrambled control. Luciferase values are the means of four separate experiments performed in triplicate (n = 12). Error bars are SEM. (iii) Semiquantitative RT-PCR of MyoD, myogenin, and GAPDH transcript levels in murine C2C12 cells after treatment with either 25 nmol each of four siRNA complementary to ERF (left lanes, 1–3) or 100 pmol (right lanes, 1–3) of an unrelated, scrambled control egg oligomer and assayed after 24 h. The – marked lane shows a negative control for RT-PCR where reaction was performed without template. No significant changes in MyoD or myogenin transcript levels were noted. Gels show results of three separate experiments. (B) Chromatin immunoprecipitation analysis of the utrophin-A promoter with ERF antibodies in C2C12 cells, demonstrating changes in ERF occupancy of the utrophin-A promoter upon treatment with MEK inhibitor U0126 and HRG treatment for 15 min. (i) RT-PCR of utrophin-A promoter from ERF-precipitated chromatin from C2C12 cells. (ii) Quantification of changes in ERF occupancy compared with the untreated ERF controls shows increased (1.63-fold) and decreased (0.64-fold) ERF levels with MEK inhibitor U0126 and HRG, respectively. Controls incubated without antibodies are shown below.

ChIP Analysis Demonstrates ERF Association with the Utrophin-A Promoter
To independently validate the interaction between ERF and theutrophin-A promoter and the role of MEK and heregulin in modulatingthe promoter (Gramolini et al., 1999a

; Khurana et al., 1999

),we used anti-ERF antibodies to perform ChIP analysis of theutrophin-A promoter in C2C12 cells that had been treated withMEK inhibitor U0126 or heregulin for 15 min or left untreated.As shown in Figure 3B, ERF was associated with the utrophin-Apromoter, and its levels were modulated by U0126 and heregulin.Consistent with the gel shift assays, subcellular localizationand reporter assays (Figure 2) as well as previous literatureon heregulin-mediated utrophin promoter activation (Gramoliniet al., 1999a

; Khurana et al., 1999

), MEK inhibitor U0126 increased,and conversely heregulin decreased, the levels of ERF associatedwith the utrophin-A promoter, respectively.

Utrophin, GABP ${alpha}$ , and ERF Expression during Development
To address the approximately eightfold perinatal reduction ofutrophin levels that leads to relatively low levels (typically0.01% of message) in the adult compared with embryonic muscle(Khurana et al., 1990, 1991), we analyzed utrophin, GABP ${alpha}$ , andERF transcript levels by using semiquantitative RT-PCR at sixtimes from embryonic day 16- (e16) to adult (1-yr)-old mdx mousehindlimb muscle (Figure 4). Utrophin and GABP ${alpha}$ transcripts weremost abundant during embryogenesis (e16), and they showed adecline of 2.5- and 1.7-fold, respectively, by perinatal day2 (p2). Analysis of adult muscle indicated that transcriptshad decreased to 11.6-fold for utrophin and 12.1 for GABP ${alpha}$ fromvalues obtained during embryogenesis (Figure 4B). Interestingly,ERF transcript levels remained high from late embryogenesisto adult muscle similar (cf. 4.9 and 5.1, respectively), withthe highest level detected at p14 (5.74 arbitrary units standardizedto GAPDH).

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Figure 4. Transcript levels of GABP ${alpha}$ , utrophin, and ERF in mdx mouse muscle. Semiquantitative RT-PCR of utrophin, GABP ${alpha}$ , ERF, and control GAPDH transcript levels at various times from embryonic day 16 to adult (12-mo-old) muscle. Utrophin and GABP ${alpha}$ transcripts are shown after a 48-h exposure, and GAPDH and ERF are shown after 24-h exposure. The graph illustrates arbitrary units of each PCR product measured by ImageQuant Tool software and expressed as a ratio to GAPDH at each time point after 24-h exposure. Left y-axis refers to ratios to GAPDH obtained for utrophin and GABP ${alpha}$ , and right y-axis refers to ERF:GAPDH ratios. E, embryonic; p, perinatal.

ERF Expression Is Localized Extrasynaptically in Adult Limb Muscle
To understand the mechanisms behind the spatially restrictedexpression of utrophin at NMJs in adult myofibers, we used LCMto selectively study gene expression levels in synaptic versusextrasynaptic regions in adult rat TA muscle (Figure 5). Demonstratingthe sensitivity and specificity of this approach, we found evidencefor highly enriched transcription at the synapse for the well-knownsynaptic markers ${alpha}$ subunit of nACHR or Chrna1 (163-fold), utrophin(7.9-fold), and Ets1 (17.9-fold). Interestingly, ERF expressionwas not detected at the synapse; however, it was exclusivelyexpressed extrasynaptically in TA muscle in vivo (Figure 5B).

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Figure 5. ERF expression is restricted exclusively to extrasynaptic regions in muscle, suggesting a role in utrophin repression. (A) Microdissection steps of synaptic and extrasynaptic regions of rat TA muscle. Cryosections of 10 µm (TA) are stained with Karnowsky and Root's method to show NMJ localization by using PEN membrane glass slides, and they are visualized using PALM light microscopy at 20x power. (A and D) Visualization of TA tissue before LCM. (B and E) Same slide cut by laser for synaptic and nonsynaptic tissue parts intending to capture. (C and F) Section visualized post-LCM, showing removal of synaptic and nonsynaptic material by catapulting to the extraction buffer. Bars, 100 µm. (B) Taqman qRT-PCR amplification plots of Chrna1 (muscle), Utrn, Ets1, Erf, and $beta$ -actin are shown on the left side of Figure 5B. The x-axis shows PCR cycle numbers up to 40, and the y-axis illustrates the ${Delta}$ of normalized reporter fluorescence dye ( ${Delta}$ Rn), which refers to new product formation in each cycle. Color codes used refer to $beta$ -actin in TA-synaptic (purple) and TA-nonsynaptic (green) and the gene of interest in TA-synaptic (red) and TA-nonsynaptic (blue) in PCR analysis. Relative gene expression of analysis data results for duplicate wells of each gene are shown as bar graphs with standard deviations, with a star indicating statistically significant differences. Because ERF (blue lines) did not reach threshold levels in this analysis, its expression level is illustrated as an electrophoretic agarose (1%) gel product at the end of 40 cycles. (C) Summary of the relative expression synaptic:nonsynaptic ratio for all genes is illustrated.

Direct Gene Transfer Confirms N-Box–mediated ERF Repression of the Utrophin-A Promoter In Vivo
Finally, we confirmed the ability of ERF to repress the wild-typeutrophin-A promoter in vivo by coinjecting the wild-type utrophinpromoter-A reporter plasmids with a CAT control plasmid to monitortransduction efficiency into TA muscles of 4-wk-old controlmice with control or ERF plasmids. Five days later, muscleswere harvested, RNA was extracted, and RT-PCR analysis for LacZand CAT was performed. In comparison with the control plasmid,promoter-A activation was significantly impaired by cotransfectionwith the ERF expression vector (31.5%; p < 0.01; Figure 6).To determine whether the N-box was required for ERF-mediatedrepression, we performed additional experiments by using thepUBF ${Delta}$ N-box construct as a reporter plasmid. As shown in Figure 6,ERF was unable to repress the mutant utrophin promoter lackingthe N-box motif in vivo. These results support and extend ourfindings from cultured muscle cells to skeletal muscle in vivo.

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Figure 6. Direct gene transfer demonstrates N-box–mediated utrophin-A promoter repression by ERF in vivo. Utrophin promoter-A constructs (wild type; with N-box) were coinjected with CAT (to monitor transduction efficiency) into TA muscles of 4-wk-old control mice with control (pSG5 vector) or ERF (pSG5-ERF) expression plasmid. A different cohort was injected using the mutant utrophin promoter constructs ( ${Delta}$ N-box; without N-box). Five days later, muscles were harvested, and then RNA extracted and qPCR analysis was performed. Values obtained for LacZ or luciferase are standardized relative to the amount of CAT present in the same sample, with the ERF-injected samples compared with their respective control (normalized to 100%). Student's t tests were used to analyze the data. The asterisk denotes the statistically significant (p < 0.02) decrease in promoter-A activation ( $~$ 30%) observed with the ERF plasmid (black bar) versus the control injected plasmid (white bar). No significant differences were observed using the ${Delta}$ N-box construct. Error bars represent SEM; sample size for wild type, n = 5; ${Delta}$ N-box, n = 10 for both ERF and control experiments.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In this study, we used gel shift (Figure 1), utrophin-A promoterreporter assays and monitoring of ERF subcellular translocationstudies (Figure 2), siRNA-mediated knockdown studies and ERF-utrophinpromoter ChIP analysis (Figure 3), in vitro expression/developmentaltime course (Figure 4) qPCR expression/localization in muscle(Figure 5), and direct gene transfer analysis (Figure 6) toidentify and characterize ERF-mediated repression as a novelmechanism for regulation of the utrophin-A promoter at a transcriptionallevel.

This study addresses a fundamental question in molecular andcellular biology—how to achieve selective localizationof genes/gene products such as ACHR or utrophin at synapses.In skeletal muscle, the problem is more extreme (than in neurons),because muscle is composed of elongated multinucleated cells,and the muscle synapse or NMJs occupy only an extremely smallportion of the cell membrane; yet, synaptic localization isachieved with considerable fidelity. Although subsynaptic transcriptionplays an important role in enriching genes such as AChR andutrophin at the NMJ (Schaeffer et al., 2001), we suggest thatthe converse mechanisms of extrasynaptic silencing may playan important role as well. ERF-mediated repression providesa novel molecular mechanism contributing to concurrent extrasynapticsilencing that must occur to achieve NMJ localization of utrophin-Ain muscle. Because ERF expression seems to be exclusively extrasynapticin TA rat muscle (Figure 5), we postulate that within theseregions (or in unstimulated muscle), low levels of utrophintranscription exist, in part, due to occupation of the N-box/EBSsite by ERF that may serve as a constitutive damper of expression(Figure 7). However, the repression is repressed at synapticregions (or when stimulated by neurite-associated HRG). On bindingof HRG to the HER 2,3,4 receptors at the NMJ, ERK is activatedby MEK-dependent phosphorylation, leading to nuclear localizationand facilitating two events, each of which favor increased utrophintranscription to occur: 1) multiple serine/threonine residuephosphorylation of ERF, causing MEK-dependent nuclear exportand a loss of repressor activity, hence derepressing the promoter(or making it more likely to be activated); and 2) activationof GABP ${alpha}$ / $beta$ , leading to greater N-box/EBS binding as well as synergisticactivation of the utrophin promoter with Sp1. Consistent withthis, ERK immunoprecipitated from HRG-treated C2C12 cells phosphorylatedERF in a MEK-dependent manner by using in vitro kinase assays(unpublished observations).

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Figure 7. Model for transcriptional regulation of utrophin promoter- A via the N-box/EBS site in muscle. Transcriptional model of the utrophin-A promoter pre- and post-ERK nuclear localization by HRG stimulation at the NMJ. Multiple arrows represent increased transcription. P, phosphorylated protein; dotted and full arrowed lines represent potential and defined signaling cascades, respectively. For more information, please refer to the text.

In conclusion, we have identified promoter repression as a novelmechanism that leads to utrophin down-regulation in extrasynapticregions of skeletal muscles. We think that derepressing thepromoter by blocking the activity of repressor molecules (suchas ERF or ERF-like molecules) either alone or in concurrencewith positively trans-activating ETS family members may be afunctional means to synergistically enhance utrophin promoteractivation as a therapeutic strategy for DMD. However, it isimportant to test these hypotheses in vivo before assigningthese important roles to the ERF transcription factors.

ACKNOWLEDGMENTS

We thank Dr. G. Mavrothalassitis, Prof. K. Davies, and Prof.A. Rosmarin for providing constructs and antibodies used inthis study. We also thank Drs. C. Bonnemann, S. Bogdanovich,and T.O.B. Krag (University of Pennsylvania) for experimentaland manuscript advice. This study was supported by grants fromthe Muscular Dystrophy Association, National Institutes of Health(AR-048871), and the Canadian Institute of Health Research.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E06-12-1069)on May 16, 2007.

Present address: Sir William Dunn School of Pathology, Universityof Oxford, Oxford, OX1 3RE, United Kingdom.

Address correspondence to: Tejvir S. Khurana (tsk{at}mail.med.upenn.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Andres, M. E., Burger, C., Peral-Rubio, M. J., Battaglioli, E., Anderson, M. E., Grimes, J., Dallman, J., Ballas, N., and Mandel, G. (1999). CoREST: a functional corepressor required for regulation of neural-specific gene expression. Proc. Natl. Acad. Sci. USA 96, 9873–9878.[Abstract/Free Full Text]

Ballas, N. et al. (2001). Regulation of neuronal traits by a novel transcriptional complex. Neuron 31, 353–365.[CrossRef][Medline]

Budak, M. T., Bogdanovich, S., Wiesen, M. H., Lozynska, O., Khurana, T. S., and Rubinstein, N. A. (2004). Layer-specific differences of gene expression in extraocular muscles identified by laser-capture microscopy. Physiol. Genomics 20, 55–65.[Abstract/Free Full Text]

Burton, E. A., Tinsley, J. M., Holzfeind, P. J., Rodrigues, N. R., and Davies, K. E. (1999). A second promoter provides an alternative target for therapeutic up-regulation of utrophin in Duchenne muscular dystrophy. Proc. Natl. Acad. Sci. USA 96, 14025–14030.[Abstract/Free Full Text]

Cerletti, M. et al. (2003). Dystrophic phenotype of canine X-linked muscular dystrophy is mitigated by adenovirus-mediated utrophin gene transfer. Gene Ther 10, 750–757.[CrossRef][Medline]

Chakkalakal, J. V., Harrison, M. A., Carbonetto, S., Chin, E., Michel, R. N., and Jasmin, B. J. (2004). Stimulation of calcineurin signaling attenuates the dystrophic pathology in mdx mice. Hum. Mol. Genet 13, 379–388.[Abstract/Free Full Text]

Chakkalakal, J. V., Stocksley, M. A., Harrison, M. A., Angus, L. M., Deschenes-Furry, J., St-Pierre, S., Megeney, L. A., Chin, E. R., Michel, R. N., and Jasmin, B. J. (2003). Expression of utrophin A mRNA correlates with the oxidative capacity of skeletal muscle fiber types and is regulated by calcineurin/NFAT signaling. Proc. Natl. Acad. Sci. USA 100, 7791–7796.[Abstract/Free Full Text]

Chaubourt, E., Fossier, P., Baux, G., Leprince, C., Israel, M., and De La Porte, S. (1999). Nitric oxide and l-arginine cause an accumulation of utrophin at the sarcolemma: a possible compensation for dystrophin loss in Duchenne muscular dystrophy. Neurobiol. Dis 6, 499–507.[CrossRef][Medline]

Clerk, A., Morris, G. E., Dubowitz, V., Davies, K. E., and Sewry, C. A. (1993). Dystrophin-related protein, utrophin, in normal and dystrophic human fetal skeletal muscle. Histochem. J 25, 554–561.[Medline]

Dennis, C. L., Tinsley, J. M., Deconinck, A. E., and Davies, K. E. (1996). Molecular and functional analysis of the utrophin promoter. Nucleic Acids Res 24, 1646–1652.[Abstract/Free Full Text]

Falls, D. L., Rosen, K. M., Corfas, G., Lane, W. S., and Fischbach, G. D. (1993). ARIA, a protein that stimulates acetylcholine receptor synthesis, is a member of the neu ligand family. Cell 72, 801–815.[CrossRef][Medline]

Fisher, R., Tinsley, J. M., Phelps, S. R., Squire, S. E., Townsend, E. R., Martin, J. E., and Davies, K. E. (2001). Non-toxic ubiquitous over-expression of utrophin in the mdx mouse. Neuromuscul. Disord 11, 713–721.[CrossRef][Medline]

Galvagni, F., Capo, S., and Oliviero, S. (2001). Sp1 and Sp3 physically interact and co-operate with GABP for the activation of the utrophin promoter. J. Mol. Biol 306, 985–996.[CrossRef][Medline]

Gilbert, R., Nalbantoglu, J., Petrof, B. J., Ebihara, S., Guibinga, G. H., Tinsley, J. M., Kamen, A., Massie, B., Davies, K. E., and Karpati, G. (1999). Adenovirus-mediated utrophin gene transfer mitigates the dystrophic phenotype of mdx mouse muscles. Hum. Gene Ther 10, 1299–1310.[CrossRef][Medline]

Gobert Gosse, S., Bourgin, C., Liu, W. Q., Garbay, C., and Mouchiroud, G. (2005). M-CSF stimulated differentiation requires persistent MEK activity and MAPK phosphorylation independent of Grb2-Sos association and phosphatidylinositol 3-kinase activity. Cell Signal 17, 1352–1362.[CrossRef][Medline]

Gramolini, A. O., Angus, L. M., Schaeffer, L., Burton, E. A., Tinsley, J. M., Davies, K. E., Changeux, J. P., and Jasmin, B. J. (1999a). Induction of utrophin gene expression by heregulin in skeletal muscle cells: role of the N-box motif and GA binding protein. Proc. Natl. Acad. Sci. USA 96, 3223–3227.[Abstract/Free Full Text]

Gramolini, A. O., Belanger, G., Thompson, J. M., Chakkalakal, J. V., and Jasmin, B. J. (2001). Increased expression of utrophin in a slow vs. a fast muscle involves posttranscriptional events. Am. J. Physiol 281, C1300–C1309.

Gramolini, A. O., Dennis, C. L., Tinsley, J. M., Robertson, G. S., Cartaud, J., Davies, K. E., and Jasmin, B. J. (1997). Local transcriptional control of utrophin expression at the neuromuscular synapse. J. Biol. Chem 272, 8117–8120.[Abstract/Free Full Text]

Gramolini, A. O., and Jasmin, B. J. (1999). Expression of the utrophin gene during myogenic differentiation. Nucleic Acids Res 27, 3603–3609.[Abstract/Free Full Text]

Gramolini, A. O., Karpati, G., and Jasmin, B. J. (1999b). Discordant expression of utrophin and its transcript in human and mouse skeletal muscles. J. Neuropathol. Exp. Neurol 58, 235–244.[Medline]

Gyrd-Hansen, M., Krag, T. O., Rosmarin, A. G., and Khurana, T. S. (2002). Sp1 and the ets-related transcription factor complex GABP alpha/beta functionally cooperate to activate the utrophin promoter. J. Neurol. Sci 197, 27–35.[CrossRef][Medline]

Hoffman, E. P., Brown, R. H., and Kunkel, L. M. (1987). Dystrophin: the protein product of the Duchene muscular dystrophy locus. Cell 51, 919–928.[CrossRef][Medline]

Jasmin, B. J., Angus, L. M., Belanger, G., Chakkalakal, J. V., Gramolini, A. O., Lunde, J. A., Stocksley, M. A., and Thompson, J. (2002). Multiple regulatory events controlling the expression and localization of utrophin in skeletal muscle fibers: insights into a therapeutic strategy for Duchenne muscular dystrophy. J. Physiol 96, 31–42.

Khurana, T. S., and Davies, K. E. (2003). Pharmacological strategies for muscular dystrophy. Nat. Rev. Drug Discov 2, 379–390.[CrossRef][Medline]

Khurana, T. S., Hoffman, E. P., and Kunkel, L. M. (1990). Identification of a chromosome 6-encoded dystrophin-related protein. J. Biol. Chem 265, 16717–16720.[Abstract/Free Full Text]

Khurana, T. S., Rosmarin, A. G., Shang, J., Krag, T. O., Das, S., and Gammeltoft, S. (1999). Activation of utrophin promoter by heregulin via the ets-related transcription factor complex GA-binding protein alpha/beta. Mol. Biol. Cell 10, 2075–2086.[Abstract/Free Full Text]

Khurana, T. S., Watkins, S. C., Chafey, P., Chelly, J., Tome, F. M., Fardeau, M., Kaplan, J. C., and Kunkel, L. M. (1991). Immunolocalization and developmental expression of dystrophin related protein in skeletal muscle. Neuromuscul. Dis 1, 185–194.[CrossRef]

Koike, S., Schaeffer, L., and Changeux, J. P. (1995). Identification of a DNA element determining synaptic expression of the mouse acetylcholine receptor delta-subunit gene. Proc. Natl. Acad. Sci. USA 92, 10624–10628.[Abstract/Free Full Text]

Krag, T. O., Bogdanovich, S., Jensen, C. J., Fischer, M. D., Hansen-Schwartz, J., Javazon, E. H., Flake, A. W., Edvinsson, L., and Khurana, T. S. (2004). Heregulin ameliorates the dystrophic phenotype in mdx mice. Proc. Natl. Acad. Sci. USA 101, 13856–13860.[Abstract/Free Full Text]

Le Gallic, L., Sgouras, D., Beal, G., Jr, and Mavrothalassitis, G. (1999). Transcriptional repressor ERF is a Ras/mitogen-activated protein kinase target that regulates cellular proliferation. Mol. Cell. Biol 19, 4121–4133.[Abstract/Free Full Text]

Le Gallic, L., Virgilio, L., Cohen, P., Biteau, B., and Mavrothalassitis, G. (2004). ERF nuclear shuttling, a continuous monitor of Erk activity that links it to cell cycle progression. Mol. Cell. Biol 24, 1206–1218.[Abstract/Free Full Text]

Love, D. R., Hill, D. F., Dickson, G., Spurr, N. K., Byth, B. C., Marsden, R. F., Walsh, F. S., Edwards, Y. H., and Davies, K. E. (1989). An autosomal transcript in skeletal muscle with homology to dystrophin. Nature 339, 55–58.[CrossRef][Medline]

Lunyak, V. V. et al. (2002). Corepressor-dependent silencing of chromosomal regions encoding neuronal genes. Science 298, 1747–1752.[Abstract/Free Full Text]

Matsumura, K., Ervasti, J. M., Ohlendieck, K., Kahl, S. D., and Campbell, K. P. (1992). Association of dystrophin-related protein with dystrophin-associated proteins in mdx mouse muscle. Nature 360, 588–591.[CrossRef][Medline]

Miura, P., Thompson, J., Chakkalakal, J. V., Holcik, M., and Jasmin, B. J. (2005). The utrophin A 5'-untranslated region confers internal ribosome entry site-mediated translational control during regeneration of skeletal muscle fibers. J. Biol. Chem 280, 32997–33005.[Abstract/Free Full Text]

Nazarian, J., Bouri, K., and Hoffman, E. P. (2005). Intracellular expression profiling by laser capture microdissection: three novel components of the neuromuscular junction. Physiol. Genomics 21, 70–80.[Abstract/Free Full Text]

Nowak, K. J., and Davies, K. E. (2004). Duchenne muscular dystrophy and dystrophin: pathogenesis and opportunities for treatment. EMBO Rep 5, 872–876.[CrossRef][Medline]

Perkins, K. J., Burton, E. A., and Davies, K. E. (2001). The role of basal and myogenic factors in the transcriptional activation of utrophin promoter A: implications for therapeutic up-regulation in Duchenne muscular dystrophy. Nucleic Acids Res 29, 4843–4850.[Abstract/Free Full Text]

Rafael, J. A., Tinsley, J. M., Potter, A. C., Deconinck, A. E., and Davies, K. E. (1998). Skeletal muscle-specific expression of a utrophin transgene rescues utrophin-dystrophin deficient mice. Nat. Genet 19, 79–82.[CrossRef][Medline]

Rosmarin, A. G., Caprio, D. G., Kirsch, D. G., Handa, H., and Simkevich, C. P. (1995). GABP and PU. 1 compete for binding, yet cooperate to increase CD18( $beta$ 2 Integrin) transcription. J. Biol. Chem 270, 23627–23633.[Abstract/Free Full Text]

Rybakova, I. N., Patel, J. R., Davies, K. E., Yurchenco, P. D., and Ervasti, J. M. (2002). Utrophin binds laterally along actin filaments and can couple costameric actin with sarcolemma when overexpressed in dystrophin-deficient muscle. Mol. Biol. Cell 13, 1512–1521.[Abstract/Free Full Text]

Sapru, M. K., Florance, S. K., Kirk, C., and Goldman, D. (1998). Identification of a neuregulin and protein-tyrosine phosphatase response element in the nicotinic acetylcholine receptor e subunit gene: regulatory role of an ets transcription factor. Proc. Natl. Acad. Sci. USA 95, 1289–1294.[Abstract/Free Full Text]

Schaeffer, L., de Kerchove d'Exaerde, A., and Changeux, J. P. (2001). Targeting transcription to the neuromuscular synapse. Neuron 31, 15–22.[CrossRef][Medline]

Schaeffer, L., Duclert, N., Dymanus, M. H., and Changeux, J. P. (1998). Implication of a multisubunit Ets-related transcription factor in synaptic expression of the nicotinic acetylcholine receptor. EMBO J 17, 3078–3090.[CrossRef][Medline]

Segalat, L., Grisoni, K., Archer, J., Vargas, C., Bertrand, A., and Anderson, J. E. (2005). CAPON expression in skeletal muscle is regulated by position, repair, NOS activity, and dystrophy. Exp. Cell Res 302, 170–179.[CrossRef][Medline]

Sgouras, D. N., Athanasiou, M. A., Beal, G. J., Fisher, R. J., Blair, D. G., and Mavrothalassitis, G. J. (1995). ERF: an ets domain protein with strong transcriptional repressor activity, can suppress ets-associated tumorigenesis and is regulated by phosphorylation during cell cycle and mitogenic stimulation. EMBO J 14, 4781–4793.[Medline]

St-Pierre, S. J., Chakkalakal, J. V., Kolodziejczyk, S. M., Knudson, J. C., Jasmin, B. J., and Megeney, L. A. (2004). Glucocorticoid treatment alleviates dystrophic myofiber pathology by activation of the calcineurin/NF-AT pathway. FASEB J 18, 1937–1939.[Abstract/Free Full Text]

Tinsley, J., Deconinck, N., Fisher, R., Kahn, D., Phelps, S., Gillis, J. M., and Davies, K. (1998). Expression of full-length utrophin prevents muscular dystrophy in mdx mice. Nat. Med 4, 1441–1444.[CrossRef][Medline]

Tinsley, J. M. et al. (1992). Primary structure of dystrophin-related protein. Nature 360, 591–593.[CrossRef][Medline]

Tinsley, J. M., Potter, A. C., Phelps, S. R., Fisher, R., Trickett, J. I., and Davies, K. E. (1996). Amelioration of the dystrophic phenotype of mdx mice using a truncated utrophin transgene. Nature 384, 349–353.[CrossRef][Medline]

Wakefield, P. M., Tinsley, J. M., Wood, M. J., Gilbert, R., Karpati, G., and Davies, K. E. (2000). Prevention of the dystrophic phenotype in dystrophin/utrophin-deficient muscle following adenovirus-mediated transfer of a utrophin minigene. Gene Ther 7, 201–204.[CrossRef][Medline]

Weir, A. P., Burton, E. A., Harrod, G., and Davies, K. E. (2002). A- and B-utrophin have different expression patterns and are differentially up-regulated in mdx muscle. J. Biol. Chem 277, 45285–45290.[Abstract/Free Full Text]

Winder, S. J., and Kendrick, J. J. (1995). Calcium/calmodulin-dependent regulation of the NH2-terminal F-actin binding domain of utrophin. FEBS Lett 357, 125–128.[CrossRef][Medline]

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