IL-1beta  alters the expression of the receptor tyrosine kinase gene r-EphA3 in neonatal rat cardiomyocytes

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IL-1 $beta$ alters the expression of the receptor tyrosine kinase gene r-EphA3 in neonatal rat cardiomyocytes

Yun You Li, Charles F. McTiernan, and Arthur M. Feldman

Cardiovascular Research Laboratories, Division of Cardiology, University of Pittsburgh Medical Center, Pittsburgh, Pennsylvania 15213

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

To identify proinflammatory cytokine responsive genes in the myocardium, we used differential display to study RNA isolatedfrom neonatal rat cardiac myocytes treated with tumor necrosisfactor- $alpha$ (TNF- $alpha$ ) and interleukin-1 $beta$ (IL-1 $beta$ ). Sequence analysisof differential display products confirmed by reverse Northernblots revealed one clone as the partial sequence of an Eph-relatedreceptor tyrosine kinase (r-EphA3). In cardiac myocytes, 36-hexposure to TNF- $alpha$ and IL-1 $beta$ reduced r-EphA3 transcripts to 59.9%(P < 0.01) of control levels; this effect was largely dependenton IL-1 $beta$ . Western blot analysis showed that changes in r-EphA3protein levels reflect that seen for transcripts. Cardiac nonmyocytesexpressed substantially lower levels of r-EphA3. Full-length r-EphA3cDNA clone (3,077 base pair) yielded an amino acid sequence with90-98% homology to the Eph receptor human EphA3, chick EphA3,and mouse EphA3. In the adult rat, r-EphA3 transcripts were mostabundant in the heart, brain, and lung. These results suggestthat IL-1 $beta$ may exert its effect on cardiac myocytes at least inpart by altering r-EphA3 expression.

proinflammatory cytokine; differential display; cardiac myocytes

	INTRODUCTION

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CIRCULATING CONCENTRATIONS of cytokines, including tumor necrosis factor- $alpha$ (TNF- $alpha$ ) and interleukin-1 $beta$ (IL-1 $beta$ ), are significantlyelevated in patients with chronic heart failure (45). TNF- $alpha$ and IL-1 $beta$ have profound negative inotropic effects on cardiacphysiology in vitro and in vivo (14, 19, 22, 29, 35,44, 51). Additionally, these cytokines adversely regulatethe expression of proteins important in cardiac excitation-contractioncoupling, including the inhibitory guanine nucleotide regulatoryprotein G_i, the calcium regulatory proteins, and inducible nitricoxide synthase (iNOS) (9, 10, 12, 34). Although a varietyof other signaling pathways have also been implicated in mediatingvarious cytokine effects (40), the specific effects that areregulated during cardiac myocyte exposure to cytokines are notfully defined.

Proinflammatory cytokines may exert their effects on cardiac myocytes through regulation of gene expression at the transcriptlevel (44). Thus identification of cytokine-responsive genetranscripts may identify unique pathways by which the pleiotropiceffects of cytokines on the heart are regulated. A powerful approachto identify such transcripts is mRNA differential display. Thistechnique can identify multiple differentially expressed transcriptswithout a priori knowledge of the particular genes or sequences(26, 27). Differential display was first introduced in 1992as a technique for the comparison, identification, and isolationof genes differentially expressed in cells or tissues under variousconditions (27). Differential display is applicable to bothsimple and complex biological systems and has been successfullyused to identify genes that are differentially expressed in heartdisease (37, 46), cancer (24, 25), and diabetes (30).

Because the proinflammatory cytokines TNF- $alpha$ and IL-1 $beta$ elicit many similar biological activities and may act synergistically,we used differential display to assess gene expression in culturedrat cardiac myocytes treated with these two cytokines. In thisreport, we identify and characterize one such proinflammatorycytokine responsive gene as an Eph-related receptor tyrosine kinase,r-EphA3.

	MATERIAL AND METHODS

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All chemicals were purchased from Sigma (St. Louis, MO), unless otherwise stated.

Cell culture and cytokine treatment. Cardiomyocytes were isolated from ventricles of 1-day-old Sprague-Dawley rat hearts asdescribed (28). Twenty-four to thirty-six hours after the cellswere plated, experiments were initiated by addition of fresh mediacontaining 5 ng/ml recombinant mouse IL-1 $beta$ and/or 100 U/ml recombinantrat TNF- $alpha$ (both from Biosource International, Camarillo, CA) ortheir vehicle [phosphate-buffered saline (PBS)]. When necessary,fresh medium containing the same cytokines was added after 24h. For comparison of different treatment durations, initiationof treatments was staggered so that collection of the cells occurredat the same time. Experiments were terminated by removing mediaand freezing culture plates on liquid nitrogen. Plates were storedat $-$ 80°C before isolation of RNA. Cardiac nonmyocytes were preparedfrom the adherent preplated cells, prepared as described above,and cultured in the same media as for the cardiac myocytes butlacking 5-bromo-2'-deoxyuridine. After two cell passages, cytokinetreatments were initiated as described for the cardiac myocytes.

To determine the percentage of nonmyocyte cells in the cardiac myocyte preparations, cells were grown on coated glass coverslipsand stained using a monoclonal anti-sarcomeric myosin antibody(MF20; Developmental Studies Hybridoma Bank, Johns Hopkins UniversitySchool of Medicine, Baltimore, MD; University of Iowa, Iowa City,IA) in a 1:2 dilution (2). Slides were then washed with PBSand incubated with a 1:100 dilution of tetramethylrhodamine isothiocyanate-labeledgoat anti-mouse antibody (Sigma). Slides were viewed with an invertedphase immunofluorescence microscope (Nikon, Melville, NY). Assessedby this method, the cardiac myocyte preparations routinely contained>95% sarcomeric-myosin-positive cells.

All experimental procedures were carried out under sterile conditions and were in accordance with the Guide for the Care andUse of Laboratory Animals (7th ed.) of the National Research Counciland approved by the Institutional Animal Care and Use Committeeof the University of Pittsburgh.

Total RNA and poly A⁺ RNA isolation. A single-step method was used for total RNA isolation from cultured neonatal rat cardiaccells or rat tissues with guanidine isothiocyanate as described(6). Poly A⁺ RNA was isolated with PolyATtract mRNA isolation system (Promega,Madison, WI) with reference to the technical manual of the manufacturer.

mRNA reverse transcription and differential display. Complementary DNA (cDNA) was synthesized by reverse transcription asfollows. Total RNA was treated with RQ1 deoxyribonuclease (DNase)(Promega) to remove residual genomic DNA before reverse transcription.Four reverse transcription reactions were carried out for eachRNA sample with 0.25 µg total RNA in Superscript II reaction buffer(GIBCO-BRL, Frederick, MD), 10 mM dithiothreitol, 20 µM of eachdeoxynucleoside 5'-triphosphate (dNTP), and 1 µM of either T12VA,T12VC, T12VG, or T12VT oligo primers (where V = A, C, or G). Thereaction mixture was heated to 70°C for 10 min and cooled to 42°C,and 250 U of Superscript II (GIBCO-BRL) were added. After furtherreaction at 42°C for 1 h, the mixture was heated to 70°C for 5min.

mRNA differential display was performed as described (24, 26). Polymerase chain reaction (PCR) amplification of the abovecDNAs was carried out with corresponding 5'-anchored primers (T12VA,T12VC, T12VG, or T12VT oligo primers) and 3' arbitrary decamers(Operon Technologies, Alameda, CA) in the presence of $alpha$ -³⁵S-labeled dATP. For each 20-µl PCR mixture, 2 µl of the reversetranscription reaction mixture were added to 18 µl of a solutionto make a final concentration of 1 µM 5'-primer, 1 µM 3'-primer,and all four dNTPs (20 µM each). Each reaction also contained10 µCi of $alpha$ -³⁵S-dATP (1,000 Ci/mmol, NEN Life Science, Boston, MA) and 3 U ofTaq DNA polymerase (Perkin Elmer, Norwalk, CT) and was overlaidwith 30 µl of mineral oil. Amplification of RNA without reversetranscription was performed to show that the PCR was reverse transcriptiondependent. The PCR reaction parameters were as follows: denaturationat 94°C for 55 s, annealing at 40°C for 2 min, extension at 72°Cfor 60 s for 40 cycles, and finally one cycle of 72°C for 8 min.DNA sequencing loading buffer was added and heated to 94°C for4 min before loading on 7% denaturing polyacrylamide gels. Gelswere run at 75 W for 140 min, dried without fixation, and exposedto BioMax film (Eastman Kodak, New Haven, CT) for 12-36 h at roomtemperature. Repeated reactions with RNA from five untreated andfour cytokine-treated sets of cells from multiple independentpreparations were performed to confirm the reproducibility ofdifferentially displayed bands.

Cloning of the differentially displayed cDNAs. Differentially displayed bands were recovered by excising the bands of interestfrom the dried sequencing gels with careful alignment of the geland film. The gels containing the band of interest were rehydratedwith 10 µl TE [10 mM tris(hydroxymethyl)aminomethane (Tris) ·Cl, 1 mM EDTA] and boiled for 20 min. The solution was transferredto a new tube, and cDNA was precipitated with ethanol and recoveredin 10 µl TE. Four microliters of the recovered cDNA were usedfor reamplification with the corresponding primers and the samePCR parameters as used for differential display, except that thereaction volume was 50 µl and did not contain $alpha$ -³⁵S-dATP. Reamplified cDNA fragments were cloned into pCRII vectors(Invitrogen, San Diego, CA). At least 10 colonies from each ligationwere selected for preparation of plasmid DNA and further analysis.

Reverse Northern blot analysis. All plasmid DNAs were isolated by a standard alkaline/sodium dodecyl sulfate (SDS) lysis procedure.Plasmid DNAs containing inserts were denatured with 0.25 M NaOH,0.5 M NaCl for 15 min at room temperature, and then diluted into0.1× SSC (1× SSC is 0.15 M NaCl and 0.015 M sodium citrate, pH7.0), 0.125 M NaOH. Plasmid DNAs (0.3 and 0.15 µg) were blottedon to nitrocellulose membranes (Schleicher & Schuell, Keene, NH).The membranes were neutralized in 0.5 M NaCl, 0.5 M Tris · Cl,pH 7.5, dried in air, and fixed by crosslinking with ultraviolet(UV) light irradiation.

Total cDNA probes were labeled directly by reverse transcription of total RNA from cytokine-untreated or cytokine-treatedcardiac myocytes with T12VA, T12VC, T12VG, or T12VT oligo primersin the presence of [ $alpha$ -³²P]dCTP (3,000 Ci/mmol, NEN Life Science). The probes were purifiedwith a Sephadex G50 spin column. Prehybridization was done in10% dextran sulfate, 1 M NaCl, and 0.1% SDS at 58°C for 10 h.The same solution was used in hybridization with the additionof 100 µg herring sperm DNA/ml and 1.2 × 10⁶ counts per minute (cpm) probe/ml. After overnight hybridizationat 60°C, the membranes were washed with 2× SSC, 0.1% SDS at 60°C,then exposed in a PhosphorImager cassette (Molecular Dynamics,Sunnyvale, CA) for 12 h. Triplicate experiments were done, andeach of the signals was quantified by integrating the volume ofeach dot with ImageQuaNT software (Molecular Dynamics). Thosethat showed changes congruent with differential display resultswere chosen for sequence analysis.

Sequencing of the cDNA fragments of differentially displayed genes and homology search with FASTA. The differentially displayedcDNA fragment inserts were cycle sequenced with M13 universalforward primer (5'-GCC AGG GTT TTC CCA GTC ACG A-3') and reverseprimer (5'-GAG CGG ATA ACA ATT TCA CAC AGG-3'). Insert sequences[sizes ranged from 177 to 593 base pair (bp)] were used for on-linehomology search with FASTA against all submitted sequences inGenBank.

RNase protection assay. RNase protection assay (RPA) was performed with a RPA II kit (Ambion, Austin, TX) following the manufacturer'sinstructions. For the synthesis of run-off radiolabeled transcripts,plasmid DNA containing the r-EphA3 insert cloned by differentialdisplay was linearized by complete digestion with EcoR V. r-EphA3cRNA antisense probe was synthesized using T7 RNA polymerase.Total RNA from control and cytokine-treated cells was hybridizedovernight at 46°C with radiolabeled antisense r-EphA3 and $beta$ -actinprobes. Protected fragments were resolved on a 6% polyacrylamidegel after digestion with RNase A/T1. The gels were dried and exposedin a PhosphorImager cassette for 12 h, and band intensities werequantified using ImageQuaNT software. All r-EphA3 bands were normalizedto the protected fragment of $beta$ -actin in the same lane to correctfor variations in loading.

Northern blot analysis. Four micrograms of poly A⁺ mRNA was resolved in formaldehyde-agarose gels, transferred to nitrocellulosemembrane by pressure blotting, and fixed by UV crosslinking. Prehybridizationwas performed overnight at 42°C in 5× SSC, 50% formamide, 5× Denhardt'sreagent, 0.2% SDS, and 25 mM sodium phosphate, pH 6.5. Hybridizationprobes were radiolabeled to at least 1 × 10⁸ cpm/µg using a random hexamer priming kit (Boehringer Mannheim,Indianapolis, IN). Radiolabeled cDNA probes were hybridized overnightat 42°C in a solution identical to the prehybridization solution,except for the addition of 10% dextran sulfate. Membranes werewashed four times with 2× SSC, 0.1% SDS at room temperature andtwice with 0.2× SSC, 0.1% SDS at 56°C. The membrane was then exposedin a PhosphorImager cassette and quantified as described above.The same blot was stripped with 2 mM Tris · Cl, pH 8.0, 0.2 mMEDTA, 0.1% SDS at 75°C for 1 h, and reprobed with a radiolabeledglyceraldehyde-3-phosphate dehydrogenase (GAPDH) probe. Membraneswere then reexposed and quantified, and results of the cDNA hybridizationwere normalized to that of the GAPDH to correct for differencesin RNA mass and efficiency of transfer.

Western blot analysis. Control and cytokine-treated cells were lysed into RIPA buffer [1× PBS, 1% NP-40, 0.5% sodium deoxycholate,0.1% SDS, and protease inhibitor cocktail (Sigma cat. P2714)].Protein concentrations were measured using the Bradford methodwith Bio-Rad protein assay reagent (Bio-Rad, Hercules, CA). Equalamounts (120 µg) of cell lysates were separated by SDS-polyacrylamidegel (6%) electrophoresis and electroblotted onto nitrocellulosemembranes. r-EphA3 protein was probed with rabbit polyclonal immunoglobulinG (IgG; Santa Cruz Biotechnology, Santa Cruz, CA) raised againstthe synthetic peptide IISSIKALETQSKNGPVPV corresponding to thededuced h-EphA3 amino acid 965-983 (the peptide is identical tor-EphA3 corresponding region 966-984). Goat anti-rabbit IgG conjugatedwith horseradish peroxidase was used as the secondary antibody.The antibody reaction was developed using an enhanced chemiluminescencereagent (NEN Life Science).

cDNA cloning and sequence analysis of r-EphA3. The full-length cDNA of the rat Eph-related receptor tyrosine kinase gene r-EphA3was cloned with a long PCR approach (21, 23). cDNA was reversetranscribed from total RNA of neonatal rat cardiac myocytes withSuperscript II and was used as template for long PCR amplification.Two overlapping fragments of the entire coding sequence were amplifiedby using high-fidelity rTth DNA polymerase (Perkin Elmer, Norwalk,CT) with the following conditions: denaturation at 94°C for 1min and annealing and extension at 67°C for 3 min for 30 cyclesafter an initial "hot start" at 78°C for 3 min. The upstream primerfor the 2.2-kb 5'-fragment and the downstream primer for the 1.1-kb3'-fragment were designed based on the conserved regions withinthe 5'- and 3'-untranslated sequences of receptor tyrosine kinases,whereas the other primers for each of the fragments were chosenfrom the sequence of the r-EphA3 fragment cloned by differentialdisplay. The two overlapping fragments were fused together togenerate full-length cDNA by repeating the above PCR reactionsfor 30 cycles without primers and templates but mixing equimolaramounts of the two fragments into the reaction. The full-lengthcDNA was cloned into a pCRII vector, and the complete sequencewas analyzed with a 377 automatic DNA sequencer (Perkin Elmer,Applied Biosystems, Foster City, CA). The resultant sequence hasbeen deposited in GenBank (accession number U69278). The predictionof hydrophobic domains of r-EphA3 was performed with on-line TMpredprogram (16). The multiple sequence alignment was made withthe on-line program Blitz (7, 41).

Data processing and statistics. The RPA and Northern blot results were quantified with ImageQuaNT software and normalizedto that for $beta$ -actin or GAPDH signals obtained from the same lane.The Western blot films were digitized with an HP ScanJet 4C scanner(Hewlett-Packard, Englewood, CO) and then quantified with ImageQuaNTsoftware. The quantitative results were presented as percent changecompared with untreated cells. The results are given as means± SD. One-way analysis of variance was applied to compare thesechanges in different experimental groups. When a significant Fvalue was obtained, comparison among the means was made by useof the post hoc Student-Newman-Keuls analysis test. Statisticalsignificance was considered at P < 0.05.

	RESULTS

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Identification of novel proinflammatory cytokine-responsive genes by mRNA differential display. Differential display with20 arbitrary 10-nucleotide primers paired to all four T12VN primersrevealed 14 upregulated and 6 downregulated PCR products whenRNA from cardiac myocytes treated with proinflammatory cytokineswas compared with that from untreated samples (Fig. 1). Repetitiveexperiments using the same primers and different batches of totalRNA produced almost equivalent banding patterns. Fifteen bandsexcised from the differential display gel were successfully elutedand reamplified with PCR; 12 of these bands were cloned afterreamplification. For each successfully reamplified and clonedproduct, plasmid DNA was isolated from 10 individual bacterialcolonies and the expression patterns were analyzed with reverseNorthern hybridization (Fig. 2). Each of the above differentiallydisplayed bands contained a number of distinct cDNA fragmentsderived from different transcripts. Not all of the cDNA fragmentsrepresented transcripts that showed changes resembling the differentialdisplay pattern. However, from 8 of the 12 reamplified bands,at least one cloned product was in accordance with the differentialdisplay results. Some bands contained multiple gene products,each of which demonstrated differential regulation. Therefore,from eight of the reamplified bands that agree with differentialdisplay results, a total of 12 genes was identified that appearedto be true positive (Table 1).

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Fig. 1. mRNA differential display of cardiac myocytes treated with tumor necrosis factor- $alpha$ (TNF- $alpha$ ) and interleukin-1 $beta$ (IL-1 $beta$ ). Repeated reactions with RNA from 5 untreated and 4 cytokine-treated sets of cells from independent preparations of cardiac myocytes were performed to confirm the reproducibility of differentially displayed bands. A, C, G, T: differential display with 5'-anchored primers of either T12VA, T12VC, T12VG, or T12VT. First 3 lanes (left to right) in each set show differential display of mRNA from untreated control cardiac myocytes, and next 2 lanes show results from cardiac myocytes treated with TNF- $alpha$ and IL-1 $beta$ for 36 h. Arrowhead points to the band that was identified to be r-EphA3.

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Fig. 2. Reverse Northern hybridization. Equal amounts of plasmid DNA (300 ng) were applied to duplicate membranes. One membrane (left) was hybridized with a reverse transcription labeled cDNA probe derived from RNA of control cardiac myocytes, whereas the second membrane (right) was hybridized with a cDNA probe derived from RNA of cardiac myocytes treated with TNF- $alpha$ and IL-1 $beta$ . The 2 membranes were depicted such that dots at corresponding positions represented the same clone. Results shown are representative of 3 independent experiments.

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Table 1. TNF- $alpha$ - and IL-1 $beta$ -responsive genes in cardiac myocytes identified by differential display

DNA sequence analyses of the clones confirmed as having differential expression revealed that all insertions had one or bothof the flanking sequences complementary to the appropriate primerpairs. The sizes of cloned inserts ranged from 177 to 593 bp.By comparison with sequences in the GenBank database, one clone(17-4) contained a 374-bp sequence that was 93% identical to bases1945 to 2318 of the mouse Eph-related receptor tyrosine kinasem-EphA3 (38). Deduced amino acid sequence of this clone had95% identity with the corresponding region of m-EphA3. Hereafter,we identify this receptor tyrosine kinase as r-EphA3 followingthe nomenclature of the Eph Nomenclature Committee (11).

Differential regulation of r-EphA3 gene by TNF- $alpha$ and IL-1 $beta$ . In addition to differential display and reverse Northern blothybridization, RPA assay and Northern blot analyses were performedto further confirm the expression pattern of r-EphA3 in neonatalrat cardiac myocytes exposed to proinflammatory cytokines. RPAassay with the cloned 374-bp r-EphA3 probe showed downregulationof r-EphA3 transcripts by combined TNF- $alpha$ and IL-1 $beta$ treatment ofcardiac myocytes (64.1 ± 18.9% that of untreated cells, n = 13,P < 0.01). IL-1 $beta$ treatment of the cells had a similar effect (67.7± 11.9% that of untreated cells, n = 4, P < 0.01) (Fig. 3). Northernblot hybridization detected two bands of 6.5 (major) and 1.4 kb(minor) (Fig. 4A). A time course study showed a significant decreasein the 6.5-kb r-EphA3 transcript after 36 h of treatment withTNF- $alpha$ and IL-1 $beta$ (59.9 ± 16.3% that of untreated cells, n = 13,P < 0.01), whereas expression of the 1.4-kb transcript appearedunchanged. Separate treatment with TNF- $alpha$ or IL-1 $beta$ showed thatthe reduction of the 6.5-kb r-EphA3 transcripts occurred onlyin the IL-1 $beta$ -treated cells (60.3 ± 17.4% that of untreated cells,n = 10, P < 0.01, Fig. 4B).

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Fig. 3. RNase protection assay. [ $alpha$ -³²P]UTP labeled r-EphA3 antisense probe was transcribed from linearized plasmid DNA containing the r-EphA3 inserts using T7 RNA polymerase. Total RNA (27 µg) from control and cytokine-treated cells was hybridized with antisense r-EphA3 and $beta$ -actin probes. Protected fragments were resolved on a 6% polyacrylamide gel after digestion with RNase A/T1. The band intensities were quantified and normalized to the protected fragment of $beta$ -actin to correct variations in loading. A: representative RNase protection assay. Marker sizes at left are in base pairs. B: summary of quantitative data (n = 12). * P < 0.05 compared with control.

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Fig. 4. Time-dependent and differential regulation of r-EphA3 expression in cardiac myocytes by TNF- $alpha$ and IL-1 $beta$ . Northern blot analysis of r-EphA3 gene expression was carried out with 4 µg poly A⁺ RNA from rat neonatal cardiac myocytes. Blots were sequentially hybridized with r-EphA3 and glyceraldehyde-3-phosphate dehydrogenase (GAPDH) probes. Differences in RNA mass were corrected by normalizing the signal for r-EphA3 to that for GAPDH. A: time-dependent downregulation of r-EphA3. Left, representative Northern blot; right, summary of the Northern blot quantitative data (n = 6-13). B: differential effect of TNF- $alpha$ and IL-1 $beta$ on the expression of r-EphA3. Left, representative Northern blot; right, summary of quantitative data (n = 7-13). * P < 0.05 compared with control.

r-EphA3 protein expression in cardiac myocytes. Western blot with polyclonal anti-EphA3 antibodies detected a robust 130-kDasignal in whole cell lysates of cardiac myocytes, whereas this130-kDa signal was not measurable in nonmyocytes. This band wascompletely abolished by preincubating the r-EphA3 antibody withthe r-EphA3 antigenic peptide (blocking peptide). The time-dependentregulation of r-EphA3 protein reflected the changes at the mRNAlevel as measured by RPA and Northern blot analyses (Figs. 3,4, and 5A). The downregulation of r-EphA3 was observed only whenIL-1 $beta$ was present in the treatment (Fig. 5B).

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Fig. 5. TNF- $alpha$ and IL-1 $beta$ regulation of r-EphA3 protein in cardiac myocytes. Myocytes were stimulated with TNF- $alpha$ (100 U/ml) and/or IL-1 $beta$ (5 ng/ml). Whole cell lysates (120 µg) were separated by sodium dodecyl sulfate-polyacrylamide gel (6%) electrophoresis and electroblotted onto nitrocellulose membrane. r-EphA3 protein was probed with rabbit polyclonal immunoglobulin G (IgG) raised against the synthetic peptide IISSIKALETQSKNGPVPV (corresponding to the deduced r-EphA3 amino acids 966-984). Goat anti-rabbit IgG conjugated with horseradish peroxidase was used as a secondary antibody. Bands were detected using a chemiluminescence reagent. A: time-dependent effect of cytokines on the expression of r-EphA3. Note band was completely blocked by preincubating the antibody with r-EphA3 peptide. B: differential effects of TNF- $alpha$ or IL-1 $beta$ . Quantitative data presented in bar graph were obtained from 4 independent experiments. * P < 0.01 compared with control.

r-EphA3 is predominantly expressed in cardiac myocytes. Northern blot analyses were also performed to assess the expressionof r-EphA3 transcripts in cardiac nonmyocytes. Hybridization toequal amounts of RNA repetitively showed that the r-EphA3 transcriptswere expressed at much lower levels in nonmyocytes relative tocardiac myocytes (Fig. 6A). Although expression at such low levelsmade assessment of alterations in transcript levels difficult,we could not detect any alteration in r-EphA3 transcript levelsin cardiac nonmyocytes exposed to proinflammatory cytokines. Atthe protein level, r-EphA3 was detected in whole cell lysatesof cardiac myocytes, but barely detectable in nonmyocyte lysates(Fig. 6B).

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Fig. 6. r-EphA3 is predominantly expressed in cardiac myocytes. A: Northern blot analysis of equal amounts (4 µg) of poly A⁺ RNA from cardiac myocytes and cardiac nonmyocytes either untreated or treated with TNF- $alpha$ and IL-1 $beta$ detected the full-length r-EphA3 transcripts in cardiac myocytes but not in nonmyocytes. B: Western blot of 120 µg whole cell lysates with polyclonal IgG against EphA3 detected a 130-kDa band in cardiac myocytes, but not in nonmyocytes.

Cloning and characterization of r-EphA3 cDNA. To further characterize r-EphA3, we applied a PCR-based approach to clone thefull-length r-EphA3 cDNA. Using primers based on the 17-4 clonesequence and previously reported sequences for 5'- and 3'-untranslatedregions of the receptor tyrosine kinases in the Eph subfamily,two overlapping fragments of 2,241 and 1,156 bp were amplifiedfrom cDNA reverse transcribed from RNA of neonatal rat cardiacmyocytes. These two fragments were then fused by coamplificationwith PCR to yield a 3,077-bp product. All PCR reactions for thiscloning used rTth DNA polymerase to reduce amplification errors.In addition, two partial clones containing additional sequencesextending from the coding region through the putative 3'-untranslatedregion were isolated by screening a rat heart cDNA library withthe 17-4 cloned fragment. Of the 200 sequenced nucleotides thatoverlapped with the clones generated through rTth-based PCR, novariations were observed, suggesting minimal PCR-generated alterationsin nucleotide sequence. After cloning, the nucleotide sequenceof the full-length coding region together with partial 5'- and3'-untranslated sequence was determined.

The predicted translation product of this sequence shows an open reading frame of 984 amino acids (nucleotides 35-2989), yieldinga protein typical of Eph-related receptor tyrosine kinase (Fig.7). Two hydrophobic regions are consistent with a signal peptidefrom amino acid 1 to 18 and a transmembrane domain from aminoacid 542 to 564. The extracellular domain of r-EphA3, which existsbetween the signal peptide and the transmembrane region, is believedto constitute the ligand binding domain and contains characteristicstructural motifs: one immunoglobulin-like domain, two fibronectinIII-like repeats, and an enrichment of cysteine residues. Similarfeatures are found in other receptor tyrosine kinases (50).In addition, the presumed cytoplasmic domain (amino acid residues565-984) contains a characteristic protein tyrosine kinase catalyticdomain, including an Mg²⁺-ATP binding site, a catalytic loop, and a putative tyrosine autophosphorylationsite at position 780, also consistent with the structure of receptortyrosine kinases. The overall nucleotide sequence homology betweenr-EphA3 and m-EphA3 is 94%, and the deduced amino acid sequencehomology is 97.5% to m-EphA3, 96% identity to h-EphA3 (48),and 90% identity to c-EphA3 (38).

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Fig. 7. Multiple alignments and comparison of amino acid sequence of r-EphA3 with its homologs. Deduced r-EphA3 amino acid sequence was aligned with sequences of mouse (m)-EphA3, human (h)-EphA3, and chick (c)-EphA3. Potential signal peptide and functional domains are underlined.

r-EphA3 mRNA expression in rat tissues. To further understand the relative importance of r-EphA3 in the heart, the expressionof r-EphA3 in various neonatal and adult rat tissues was studiedby Northern blot analysis. The 6.5-kb full-length transcript wasmost prominent in adult brain, heart, and lung (Fig. 8). It wasexpressed in both neonatal and adult rat hearts. Other tissues,such as lung and kidney, showed developmental alterations in theexpression of the r-EphA3 gene. The 1.4-kb transcript was mostprominent in neonatal skeletal muscle tissue. Subsequent attemptsto find an r-EphA3 transcript corresponding to the 1.4-kb bandby rapid amplification of cDNA ends, screening of a rat heartcDNA library, and slot blot analyses with selected regions ofthe r-EphA3 cDNA suggested that the 1.4-kb transcript did notarise from an alternatively spliced product of the r-EphA3 gene(data not shown).

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Fig. 8. Tissue distribution of r-EphA3 mRNA. A multiple tissue Northern blot containing ~4 µg of poly A⁺ RNA from rat neonatal and adult tissues indicates greatest r-EphA3 expression is in the heart, brain, and lung. Blot was probed with GAPDH to ensure that the RNA in each lane was intact. A: neonatal tissues. B: adult tissues.

	DISCUSSION

Top Abstract Introduction Methods Results Discussion References

Use of differential display to identify novel cytokine-responsive genes in cardiac myocytes. Differential display is a methodwith great potential for discovering alteration in gene expressionand novel gene transcripts. The high sensitivity of this techniquemakes it prone to false positives; therefore, it is necessaryto repeat the same experiment with multiple samples and to verifydifferentially displayed genes by complementary methods. For thispurpose we repeated differential display with RNA from differentpreparations of cytokine-treated cell cultures and identifiedsimilar changes in the pattern of amplified products. The reverseNorthern blot procedure was applied to screen and analyze allthe candidate differentially displayed cDNA clones. The verifiedclones congruent with the results of differential display wereused in RPA and Northern blot analyses to quantitate mRNA expression.Our results suggest that a variety of genes are differentiallyregulated when cultured cardiac myocytes are treated with proinflammatorycytokines. Indeed, in addition to a series of novel genes, wehave identified an Eph-related receptor tyrosine kinase, r-EphA3,not previously investigated in the myocardium.

r-EphA3 transcript and protein are regulated by IL-1 $beta$ in neonatal rat cardiac myocytes. Differential display identified r-EphA3as being downregulated by cotreatment with TNF- $alpha$ and IL-1 $beta$ . RPAand Northern blot analyses demonstrated that these cytokines produced~40% reduction in r-EphA3 transcript levels. This reduction wasapparently mediated by IL-1 $beta$ , as TNF- $alpha$ alone did not change theexpression of r-EphA3, whereas IL-1 $beta$ alone mimicked the effectof cotreatment of the cells with TNF- $alpha$ and IL-1 $beta$ at both the RNAand protein levels. This effect is not immediate and appears totake several hours to develop. The r-EphA3 protein changes aretemporally related to changes in transcript levels, suggestingthe r-EphA3 is transcriptionally regulated. However, the mechanismby which IL-1 $beta$ downregulates r-EphA3 transcript levels remainsunknown.

Role of Eph-related receptor tyrosine kinases in response to proinflammatory cytokines. The Eph family of receptors constitutesthe largest subgroup of the receptor tyrosine kinases family (47).The functional significance of the Eph subfamily of receptor tyrosinekinases is not well defined. Some (including m-EphA3, the murinehomologue of r-EphA3) may play a role in signal transduction duringdifferentiation, development, carcinogenesis, neuron axon bundleformation, and control of cytoskeletal architecture (15, 17,49). Amino acid sequence comparisons demonstrated very highhomology among r-EphA3 and mouse (m-EphA3), chick (c-EphA3), andhuman (h-EphA3) receptor tyrosine kinases, implying a similarfunction among these genes. The identification of r-EphA3 as acytokine-responsive gene in cardiac myocytes suggests the presenceof additional roles for Eph receptors in both inflammation andcardiac diseases.

It is of interest to note that B61, the prototypic member of the family of ligands for Eph receptors, was first identifiedas a protein whose expression was upregulated in response to TNF- $alpha$ (3). Indeed, B61 has been proposed to participate in the angiogenesisassociated with inflammation (36). In addition to these studieswith B61, several additional observations suggest that receptortyrosine kinases including r-EphA3 might participate in cytokinesignal processing: 1) IL-1 $beta$ -inducible expression of gro- $beta$ andiNOS are dependent on tyrosine kinase signaling pathways (8,20, 39, 43), 2) cytokines can induce rapid tyrosine phosphorylationof several signaling molecules through tyrosine kinases (42),3) the effect of IL-1 $beta$ on the hypertrophic growth of neonatalrat cardiac myocytes can be blocked by the tyrosine kinase inhibitorgenistein (44), and 4) this report observed that IL-1 $beta$ exposureproduces significant decrease in r-EphA3 expression in cardiacmyocytes at both the transcript and protein levels, although thepathway by which this occurs is unclear. Because the signal transductionpathways activated through EphA3 are unknown, it is unclear howor even whether a 50% reduction in the level of r-EphA3 proteinmay alter cell and organ physiology. It is reported that IL-1 $beta$ induces hydrolysis of GTP (32, 33), and the activation ofthe related Eph receptor EphB2 leads to multiple and sequentialkinase reactions and modulates hydrolysis of GTP by regulatingthe activities of Ras-GTPase activating protein (17, 18).Thus it is possible that IL-1 $beta$ -induced changes in the level ofr-EphA3 could significantly modify downstream signal transductioncascades and cellular physiology through a similar pathway. Wenote that, by analogy, a 50% reduction in the level of $beta$ ₁-adrenergicreceptor is found in the failing human myocardium and is associatedwith profound functional alterations (4, 5).

Tissue distribution of r-EphA3 transcripts. Having demonstrated that r-EphA3 was an IL-1 $beta$ -responsive gene in neonatal ratcardiac myocytes, we isolated full-length cDNA clones to moredefinitively identify the potential protein that this transcriptencodes and examined the tissue-specific expression of r-EphA3transcripts. We found that r-EphA3 is expressed in both neonataland adult rat hearts. Additionally, some organs (such as lungand kidney) show marked differences in the expression of r-EphA3between the neonatal and adult organism (Fig. 8). However, thefunction of this receptor tyrosine kinase in the heart remainsundefined. In other organs, receptor tyrosine kinases play a rolein cellular differentiation and proliferation (1, 13, 31).As cardiac myocytes are terminally differentiated nonproliferativecells, the signaling events mediated by r-EphA3 may stimulateresponses other than mitogenesis or differentiation.

In conclusion, differential display identified the r-EphA3 receptor tyrosine kinase as an IL-1 $beta$ -responsive gene in neonatalcardiac myocytes. r-EphA3 expression is downregulated in cardiacmyocytes at both the mRNA and protein levels after 36-h treatmentof the cells with IL-1 $beta$ . This receptor and other members of theEph-receptor family have not been previously studied in the myocardium.Our results suggest that IL-1 $beta$ may exert its effects on cardiacmyocytes at least in part by modulating r-EphA3 expression. However,the physiological relevance of the ~50% reduction in r-EphA3 expressionand the pathway by which IL-1 $beta$ alters r-EphA3 expression remainto be determined.

	ACKNOWLEDGEMENTS

We thank Bonnie Lemster for help with the cell preparations.

	FOOTNOTES

Address for reprint requests: C. F. McTiernan, 1744.1 Biomedical Science Tower, Division of Cardiology, Univ. of Pittsburgh Medical Center, 200 Lothrop St., Pittsburgh, PA 15213.

Received 17 June 1997; accepted in final form 24 September 1997.

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IL-1 alters the expression of the receptor tyrosine kinase gene r-EphA3 in neonatal rat cardiomyocytes

IL-1 $beta$ alters the expression of the receptor tyrosine kinase gene r-EphA3 in neonatal rat cardiomyocytes