Role of protein kinase C-{epsilon} in hypertrophy of cultured neonatal rat ventricular myocytes

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Role of protein kinase C- $epsilon$ in hypertrophy of cultured neonatal rat ventricular myocytes

James B. Strait III¹, Jody L. Martin¹, Allison Bayer¹, Ruben Mestril¹, Diane M. Eble², and Allen M. Samarel¹^,²

The Cardiovascular Institute and the Departments of ¹ Physiology and ² Medicine, Loyola University Chicago Stritch School of Medicine, Maywood, Illinois 60153

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Using adenovirus (Adv)-mediated overexpression of constitutively active (ca) and dominant-negative (dn) mutants, we examinedwhether protein kinase C (PKC)- $epsilon$ , the major novel PKC isoenzymeexpressed in the adult heart, was necessary and/or sufficientto induce specific aspects of the hypertrophic phenotype in low-density,neonatal rat ventricular myocytes (NRVM) in serum-free culture.Adv-caPKC- $epsilon$ did not increase cell surface area or the total protein-to-DNAratio. However, cell shape was markedly affected, as evidencedby a 67% increase in the cell length-to-width ratio and a 17%increase in the perimeter-to-area ratio. Adv-caPKC- $epsilon$ also increasedatrial natriuretic factor (ANF) and $beta$ -myosin heavy chain (MHC)mRNA levels 2.5 ± 0.3- and 2.1 ± 0.2-fold, respectively, comparedwith NRVM infected with an empty, parent vector (P < 0.05 forboth). Conversely, Adv-dnPKC- $epsilon$ did not block endothelin-inducedincreases in cell surface area, the total protein-to-DNA ratio,or upregulation of $beta$ -MHC and ANF gene expression. However, thedominant-negative inhibitor markedly suppressed endothelin-inducedextracellular signal-regulated kinase (ERK) 1/2 activation. Takentogether, these results indicate that caPKC- $epsilon$ overexpression alterscell geometry, producing cellular elongation and remodeling withouta significant, overall increase in cell surface area or totalprotein accumulation. Furthermore, PKC- $epsilon$ activation and downstreamsignaling via the ERK cascade may not be necessary for cell growth,protein accumulation, and gene expression changes induced byendothelin.

endothelin-1; extracellular signal-regulated kinase; signal transduction; heart; adenovirus

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

HYPERTROPHIC GROWTH is a common response of the myocardium to ischemic injury, hypertension, or valvular and congenital heartdisease. Although the chronically increased wall stress that accompaniesthese disorders results in an initially beneficial adaptationto maintain normal cardiac function, the development of left ventricularhypertrophy (LVH) poses an independent risk factor for subsequentcardiovascular morbidity and mortality (3). Hypertrophic cardiacgrowth is characterized by the activation of various cell signalingkinases, the induction of immediate early gene expression, thereexpression of a fetal gene program of secondary response genes,and the ultimate development of increased cardiomyocyte cell volumeand protein accumulation in the absence of cell division. Despitea wealth of experimental and clinical data regarding the developmentand progression of cardiac hypertrophy, the intracellular mechanismswhereby cardiomyocytes sense the increased hemodynamic load andconvert mechanical stimuli into growth-promoting biochemical processesare only now beingelucidated.

Investigators interested in the signal transduction cascades responsible for the induction of cardiomyocyte hypertrophy havemade extensive use of cultured neonatal rat ventricular myocytes(NRVM). These cells display many characteristics of the hypertrophicphenotype when subjected to either neurohormonal or mechanicalstimuli that induce cardiomyocyte hypertrophy in vivo (42).A common feature of many of these hypertrophic stimuli is theactivation of one or more of the isoenzymes of protein kinaseC (PKC). PKCs are a family of phospholipid-dependent, serine-threoninekinases that are divided into three subfamilies (conventional,novel, and atypical) based on their activation requirements forCa²⁺ and diacylglycerol and their sensitivity to phorbol esters. ThePKC family includes at least twelve members. NRVM express onlyPKC- $alpha$ , PKC- $delta$ , PKC- $zeta$ , and PKC- $epsilon$ (35), which may be differentiallyregulated and have specific functions in the cardiomyocyte (31).This specificity is likely due to their differential activationby hypertrophic stimuli (5, 13, 31) and their differentiallocalization within the cell (16). Nevertheless, the role ofeach isoenzyme in the induction of specific aspects of the hypertrophicphenotype remainsunknown.

PKC- $epsilon$ is one of the three phorbol-ester-sensitive PKC isoenzymes found in NRVM and is the most abundant novel (i.e., Ca²⁺-insensitive) PKC isoenzyme found in adult rat cardiac myocytes(5). Previous studies investigating the importance of PKC- $epsilon$ in cardiomyocyte hypertrophy have demonstrated that, of the majorPKC isoenzymes expressed in rat cardiomyocytes, only PKC- $epsilon$ translocatesin response to acute pressure overload (27). Additionally, Clerket al. (13) and Jiang et al. (24) have suggested that PKC- $epsilon$ is an upstream regulator of the Ras-Raf-mitogen/extracellularsignal-regulated kinase (MEK)-extracellular signal-regulated kinase(ERK) signaling cascade. This signal transduction pathway hasbeen implicated in mediating both cardiomyocyte gene expressionchanges and cytoskeletal alterations in response to hypertrophicagonists (1, 10, 20, 21, 29, 44, 45). On the basisof these previous reports, the objective of the present studywas to utilize adenoviral vectors expressing constitutively activeand dominant-negative mutants of PKC- $epsilon$ to critically analyze whetherthis signaling kinase is necessary and/or sufficient for the inductionof specific aspects of the cardiomyocyte hypertrophicphenotype.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Reagents. PC-1 tissue culture medium was obtained from BioWhittaker (Walkersville, MD). DMEM was obtained from GIBCO-BRL (Grand Island,NY). Medium 199, Ca²⁺-free and Mg²⁺-free Hanks' balanced salts (HBSS; modified), acid-soluble calfskin collagen, and antibiotic/antimycotic solution were obtainedfrom Sigma Chemical (St. Louis, MO). Permanox chamber slides wereobtained from Nunc (Naperville, IL). [³²P]ATP and [³²P]dCTP were purchased from Amersham (Arlington Heights, IL). Monoclonalantibodies to PKC- $epsilon$ and paxillin were obtained from Signal TransductionLaboratories (Lexington, KY). Rabbit polyclonal antibodies toERK1 and ERK2 were obtained from Santa Cruz Biotechnology (SantaCruz, CA). Rabbit polyclonal antibodies to the phosphorylatedforms of ERKs were obtained from Promega (Madison, WI). Goat anti-mouserhodamine-conjugated IgG and FITC-phalloidin were obtained fromMolecular Probes (Eugene, OR). Horseradish peroxidase-conjugatedgoat anti-rabbit and goat anti-mouse IgGs were from Bio-Rad (Hercules,CA). PKC- $epsilon$ specific substrate peptide (Glu-Arg-Met-Arg-Pro-Arg-Lys-Arg-Gln-Gly-Ser-Val-Arg-Arg-Arg-Val)was obtained from Biomol (Plymouth Meeting, MA). All other reagentswere of the highest grade commercially available and were obtainedfrom Sigma and Baxter (McGaw Park,IL).

Adenoviral constructs. Constitutively active (ca) PKC- $epsilon$ adenovirus (Adv) was constructed by first subcloning caPKC- $epsilon$ cDNA (kindly provided by Drs.Peter Parker and Peter Sugden, Imperial College of Science Technologyand Medicine, Cambridge, UK) into a pAC-CMV-pLpA-SR (SR) plasmid.The enzyme was made constitutively active by deletion of residues154-163 of its inhibitory pseudosubstrate domain (47). The subclonedconstruct was then cotransfected along with pJM17 plasmid thatcontained adenoviral DNA into HEK-293 cells. After homologousrecombination, the recombinant Adv was plaque-purified and amplified.Dominant-negative (dn) PKC- $epsilon$ Adv was kindly provided by Dr. PeipeiPing, University of Louisville Medical School (Louisville, KY)and constructed as previously described (30). Briefly, the mutantcDNA was constructed by first obtaining the full-length cDNA froma rabbit heart cDNA library using a cDNA probe provided by Dr.Shigeo Ohno (Yokohama City University, Yokahama, Japan). A humanhemagglutinin epitope tag was added to the 5'-end of the rabbitcDNA through site-directed mutagenesis. The construct was thenmutated at the ATP-binding site [amino acid 436 (K to R)] andits pseudosubstrate domain [amino acid 159 (A to E)], therebydestroying the construct's kinase activity but maintaining theenzyme in an active conformation. The double-mutant PKC- $epsilon$ wasthen used in the generation of a replication-defective Adv asdescribed above. Adv were amplified and purified using HEK-293cells, as previously described (18). Viral titers were estimatedby absorbance at 260 nm (A₂₆₀): viral particles/ml = A₂₆₀ × dilution× 10¹⁰ (2).

Ventricular dissociation and cardiac myocyte isolation. Animals used in these experiments were handled in accordance with the Guiding Principles in the Care and Use of Animals, approvedby the Council of the American Physiological Society. Ventricularmyocytes were isolated from the hearts of 2-day-old Sprague-Dawleyrats by collagenase digestion, as previously described (36).Released cells were collected by centrifugation, resuspended inPC-1 medium, plated at a density of 400 cells/mm² on collagen-coated tissue culture dishes or chamber slides, andleft undisturbed in a 5% CO₂ incubator for 14-18 h. Unattachedcells were removed by aspiration and washed two times in HBSS,and the attached cells were maintained in a solution of DMEM-medium199 (4:1) containing antibiotic/antimycotic solution. Thereafter,media were changed daily. Cardiomyocytes were infected (60 min,25°C with gentle agitation) with various concentrations of replication-defectiveAdv diluted in DMEM-medium 199. Medium was then replaced withvirus-free DMEM-medium 199, and the cells were cultured for anadditional 48-72 h. Under these cell culture conditions, cardiomyocytesdisplay little or no spontaneous intracellular Ca²⁺ concentration ([Ca²⁺]_i) transients or beating activity (18, 19).

Surface area and cell shape analysis. Cardiomyocytes were loaded with 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein (BCECF)-AM [2 µM in a modified Krebs medium(in mM: 135 NaCl, 5.9 KCl, 1.5 CaCl₂, 1.2 MgCl₂, 11.5 glucose,and 11.6 HEPES, pH 7.3) supplemented with 0.1% BSA and 0.02% PluronicF-127 detergent] for 1 h followed by incubation in BCECF-freeKrebs buffer for 1 h. Cells were then viewed using a Zeiss modelLSM 410 laser scanning confocal microscope. Optical sections throughthe bottom of the cells (~10 cells/field) were then stored, andthe digital images were subjected to image analysis using theImage-1 Software Package (Universal Imaging, West Chester, PA).A binary mask was created by setting a threshold brightness thatdistinguished the fluorescent cells from the black background.The area of each cell was then determined as an exact count ofthe number of pixels that make up the object's binary mask multipliedby the area of a unit pixel. Cell perimeter was measured as thelength of the outline of the object's binary mask. The shape factorclassified objects based on the extent of their roundness, whichwas derived from the measured perimeter and area of the object'sbinary mask, and was calculated according the to following formula

shape factor<IT>=</IT>[(<IT>4&pgr;a</IT>)<IT>&cjs0823; p<SUP>2</SUP></IT>]

where p is the perimeter in µm, and a is the area in µm².

Immunofluorescence. Cells grown on Permanox chamber slides were fixed (10 min, room temperature) with 2% (wt/vol) paraformaldehyde in sodium PBS,washed (15 min) in 1% (wt/vol) glycine in PBS, and permeabilized(15 min) with 0.5% (vol/vol) Triton X-100 in PBS. Samples werefirst incubated in blocking solution (PBS + 0.1% Triton X-100+ 1% goat serum) for 1 h. Myocytes were then stained with anti-paxillinmonoclonal antibody (1:1,000 in blocking solution) for 1 h andthen were stained with a rhodamine-conjugated, donkey anti-rabbitsecondary antibody (1:30 in blocking solution) for 1 h. Cellswere also stained with FITC-conjugated phalloidin (1:40 in PBS)for 1 h to visualize F-actin filaments and myofibrillar structure.The stained cells were viewed using a Zeiss model LSM 510 laserscanning confocal microscope. Multiple optical sections ~1 µMthick were taken of each sample to eliminate out-of-focus fluorescenceof the intensely stainedmyocytes.

Cellular composition. For the quantitative analysis of total cellular protein and DNA content, 0.2 N perchloric acid (1 ml) was added, and the cellswere then scraped from the dishes and collected by centrifugation(10,000 g, 10 min). The precipitate was redissolved by incubation(60°C, 20 min) in 250 µl of 0.3 N KOH. Aliquots were then usedfor analysis of total protein by the Lowry method using crystallinehuman serum albumin as standard and for DNA using 33258 Hoechstdye and salmon sperm DNA as standard, as previously described(36). Data were the means of duplicate wells for each cell isolationand were expressed as microgram total protein per microgramDNA.

mRNA analysis. Total cellular RNA was isolated by the method of Chomczynski and Sacchi (11). RNA was quantified by absorbance at 260 nm,and its integrity was determined by examining the 28S and 18SrRNA bands in ethidium bromide-stained agarose gels. Rat $alpha$ -myosinheavy chain (MHC), $beta$ -MHC, atrial natriuretic factor (ANF), andsarco(endo)plasmic reticulum Ca²⁺-ATPase (SERCA) 2 mRNAs and rat 18S rRNA were then quantitativelyanalyzed by Northern blotting and scintillation spectroscopy (InstantImager, Hewlett-Packard), as previously described (8).

Subcellular fractionation. Subcellular fractionation was performed as previously described (41) with minor modifications. Briefly, NRVM grown on 35-mmdishes were washed with PBS, and 200 µl of homogenization buffer(2 mM EDTA, 2 mM EGTA, 10 µg/ml aprotinin, 10 µg/ml leupeptin,500 µM sodium orthovanadate, 1 mM Pefabloc, and 20 mM Tris · HCl,pH 7.5) were added. Cells were then frozen in a dry ice-methanolbath, thawed on ice, scraped into a plastic tube, and sonicated.The cell homogenate was then centrifuged (100,000 g, 60 min, 4°C),and the supernatant fraction (representing the cytosolic fraction)was stored at $-$ 80°C. The pellet was resuspended by sonicationin 200 µl of extraction buffer (20 mM Tris · HCl, pH 7.4, 2 mMEDTA, 5 mM EGTA, 0.25 M sucrose, 5 mM $beta$ -mercaptoethanol, 20 µg/mlleupeptin, 20 µg/ml aprotinin, 1 mM Pefabloc, and 0.5% TritonX-100). After centrifugation, the supernate [representing themembrane-bound (P₁) fraction] was stored at $-$ 80°C.

PKC activity assay. PKC- $epsilon$ enzyme activity was measured in total cell extracts and subcellular fractions as follows. For total cell extracts, NRVMwere scraped in 200 µl of extraction buffer (20 mM Tris · HCl,pH 7.4, 2 mM EDTA, 5 mM EGTA, 0.25 M sucrose, 5 mM $beta$ -mercaptoethanol,20 µg/ml leupeptin, 20 µg/ml aprotinin, 1 mM Pefabloc, and 0.5%Triton X-100), lysed via sonication, and centrifuged (16,000 g,30 min). Subcellular fractions were prepared as described above.The reaction mixture consisted of 25 µg of lysate protein in 20µl of PKC assay buffer [50 mM Tris · HCl, pH 7.4, 250 µg/ml BSA,1 mM EGTA, 80 µg/ml phosphatidylcholine, 20 µg/ml phosphatidylserine,7.5 mM magnesium acetate, 200 nM phorbol 12-myristate 13-acetate(PMA), and 10 µM PKC- $epsilon$ specific substrate peptide]. The reactionwas begun by the addition of 25 µM ATP (containing 0.5 µCi/assay[³²P]ATP) and incubation at 30°C for 10 min. Next, 25 µl of the reactionmixture were spotted onto a P81 phosphocellulose filter and air-dried.Filters were washed three times for 10 min each with 0.5% phosphoricacid and then one time with acetone. ³²P radioactivity was measured using a scintillationcounter.

Mitogen-activated protein kinase and PKC Western blotting. NRVM were washed one time with PBS, and 300 µl of lysis buffer (50 mM sodium pyrophosphate, 50 µM NaF, 50 µM NaCl, 5 mM EDTA,5 mM EGTA, 100 µM sodium orthovanadate, 10 µg leupeptin/ml, 10µg aprotinin/ml, 1 mM Pefabloc, 0.01% Triton X-100, and 10 mMHEPES, pH 7.4) were added. Cells were then frozen on a dry ice-methanolbath, thawed on ice, and scraped in a plastic tube. Samples weresonicated one time and centrifuged (14,000 g; 30 min), and thesupernatant fractions were stored at $-$ 80°C. ERK1/2 activationwas assessed by separating equal amounts of cellular protein (20-50µg, as determined by the bicinchoninic acid-Bradford method) bySDS-PAGE and Western blotting with polyclonal antibodies specificfor the phosphorylated forms of ERK1/2. Primary antibody bindingwas visualized using enhanced chemiluminescence and was quantifiedby laser densitometry. In some experiments, ERK1/2 activationand abundance were assessed by gel-shift analysis, as previouslydescribed (18, 41). PKC abundance was assessed using similarSDS-PAGE and Western blotting techniques, except that cells werescraped in a modified lysis buffer (150 mM NaCl, 10% glycerol,1.5 mM MgCl₂, 1 mM EGTA, 1% sodium deoxycholate, 1% Triton X-100,0.1% SDS, 10 µg/ml aprotinin, 10 µg/ml leupeptin, 500 µM sodiumorthovanadate, and 1 mM Pefabloc, pH 7.5), and nitrocellulosemembranes were probed with PKC- $epsilon$ -specific monoclonalantibodies.

Data analysis. Results were expressed as means ± SE. Normality was assessed using the Kolmogorov-Smirnov test, and homogeneity of variancewas assessed using Levene's test. Data were compared by one-wayblocked ANOVA on Ranks followed by the Student-Newman-Keuls test,paired or unpaired t-tests, or Mann-Whitney Rank Sum or WilcoxonSigned Rank tests, where appropriate. Data were analyzed usingthe SigmaStat Statistical Software Package (Jandel Scientific,San Rafael,CA).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Overexpression of caPKC- $epsilon$ alters NRVM morphology but does not induce NRVM hypertrophy. To determine whether PKC- $epsilon$ overexpression was sufficient to induce hypertrophic growth, we overexpressed PKC- $epsilon$ , which wasmade constitutively active by deletion of its pseudosubstratedomain (47). Overexpression was achieved by use of an adenoviralvector (Adv-caPKC- $epsilon$ ) that was generated in our laboratories. Infectionof NRVM with this Adv resulted in a large, dose-dependent increasein PKC- $epsilon$ immunoreactivity, as shown in the representative immunoblotin Fig. 1A. Subcellular fractionation of Adv-caPKC- $epsilon$ -infectedcells indicated that the majority of the constitutively activeenzyme was in a Triton X-100 soluble membrane fraction under basalconditions (data not shown). PKC enzyme activity was measuredin total cell extracts using a PKC- $epsilon$ -specific substrate peptide(Fig. 1B). Based on the near-maximal level of PKC- $epsilon$ activity incells infected with 100 viral particles/cell, this amount of Adv-caPKC- $epsilon$ was used in all subsequent experiments.

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Fig. 1. Overexpression of constitutively active (ca) protein kinase C (PKC)- $epsilon$ in neonatal rat ventricular myocytes (NRVM). A: NRVM were maintained under control conditions (Uninfected) or were infected with 10-1,000 viral particles/cell (ppc) of replication-defective adenovirus (Adv) encoding caPKC- $epsilon$ (Adv-caPKC- $epsilon$ ) or a control adenovirus containing no insert (Adv-SR). After 48 h, cells were harvested for analysis of immunoreactive PKC- $epsilon$ by SDS-PAGE and Western blotting with a monoclonal antibody specific for PKC- $epsilon$ . B: NRVM were infected with 10-1,000 ppc of replication-defective adenovirus encoding bacterial $beta$ -galactosidase (Adv- $beta$ gal) or Adv-caPKC- $epsilon$ . PKC- $epsilon$ enzyme activity in whole cell extracts was analyzed by ³²P incorporation using a PKC- $epsilon$ -specific peptide substrate. cpm, Counts/min.

We have previously shown that agonists that activate PKC isoenzymes, such as phenylephrine (PE), endothelin-1 (ET), and PMA,increase NRVM cell surface area and total protein content (18,32, 36, 37, 41). As shown in Table 1, however, overexpressionof caPKC- $epsilon$ alone did not increase overall cell surface area, nordid it increase total protein content or the total protein-to-DNAratio. In fact, total protein/DNA ratio actually decreased inAdv-caPKC- $epsilon$ overexpressing cells as a result of a small but significantincrease in DNA content per dish (576 ± 72 vs. 671 ± 86 ng DNA/wellfor Adv-SR vs. Adv-caPKC- $epsilon$ -infected cells, respectively; P < 0.02).Nevertheless, Adv-caPKC- $epsilon$ -infected NRVM developed a marked alterationin cell shape within 48 h of viral infection. As seen in the phase-contrastimages of live cardiomyocytes, NRVM infected with Adv-caPKC- $epsilon$ (Fig. 2B) were noticeably elongated compared with cells infectedwith equal amounts of Adv-SR (Fig. 2A). Immunocytochemical analysisof fixed and permeabilized cells revealed that NRVM infected withAdv-caPKC- $epsilon$ (Fig. 2D) retained actin filaments that traversedthe entire length of the elongated cell processes and that terminatedin paxillin-positive focal adhesions. Paxillin staining was alsoobserved in a band-like pattern along the length of the cell projections,consistent with the appearance of focal adhesions and costameres(19, 38). In contrast, Adv-SR-infected cells were irregularin shape, with individual actin filaments oriented in multipledirections within an individual cell (Fig. 2C). Paxillin stainingwas also observed along the length of the actin cables and atterminal focal adhesions.

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Table 1. Overexpression of caPKC- $varepsilon$ causes alterations in cell shape

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Fig. 2. Overexpression of caPKC- $epsilon$ alters NRVM morphology. NRVM were infected with 100 ppc Adv-SR (A and C) or Adv-caPKC- $epsilon$ (B and D). After 48 h, digital images of living myocytes were recorded using an inverted, phase-contrast microscope (×20 objective) and a Kodak DC120 digital camera (A and B). Identically treated cells were fixed, permeabilized, and stained with a mouse monoclonal antibody specific for the cytoskeletal protein paxillin (red) and with FITC-phalloidin (green) to visualize focal adhesions and actin filaments, respectively (C and D). Myocytes were then viewed using a Zeiss LSM 510 laser scanning confocal microscope (×40 objective, Zoom factor 1.0). Regions of colocalization appear yellow.

We quantified these alterations in cell shape using image analysis of BCECF-loaded, live cells, and the results of three differentexperiments are depicted in Table 1. NRVM infected with Adv-caPKC- $epsilon$ showed a 67% increase in the cell length-to-width ratio and a17% increase in the perimeter-to-area ratio. Quantification ofthe shape factor, an index of cell roundness, similarly revealedthat cells overexpressing caPKC- $epsilon$ were significantly less roundcompared with NRVM infected with Adv-SR.

Overexpression of caPKC- $epsilon$ alters ANF and MHC mRNA levels. Previous studies have shown that transient transfection of constitutively active mutants of PKC- $alpha$ , PKC- $beta$ , PKC- $epsilon$ , and PKC- $zeta$ all transactivated ANF promoter activity in NRVM (15, 39),whereas constitutively active mutants of PKC- $alpha$ and PKC- $beta$ transactivated $beta$ -MHC promoter activity, albeit to different extents (25). Allof these studies employed promoter-reporter gene constructs inlow-efficiency, transient transfection assays to analyze transcriptionalinduction of these marker genes. Therefore, as a further checkon the effects of caPKC- $epsilon$ overexpression on the induction of thehypertrophic phenotype, we examined steady-state mRNA levels of $alpha$ -MHC, $beta$ -MHC, ANF, and SERCA2 48 h after viral infection. As shownin Fig. 3, Adv-caPKC- $epsilon$ increased ANF and $beta$ -MHC mRNA levels 2.5± 0.3- and 2.1 ± 0.2-fold, respectively, compared with Adv-SR-infectedNRVM (P < 0.05 for both). In contrast, $alpha$ -MHC mRNA levels weresignificantly reduced by 43 ± 8% compared with Adv-SR-infectedcells (P < 0.05), but SERCA2 mRNA levels were unaffected (1.2± 0.1-fold change; P > 0.5).

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Fig. 3. Overexpression of caPKC- $epsilon$ alters NRVM gene expression. A: NRVM were infected with 100 ppc Adv-SR or Adv-caPKC- $epsilon$ . After 48 h, total RNA (10 µg/lane) was size-fractionated by denaturing agarose gel electrophoresis, transferred to nylon membrane, and sequentially probed with ³²P-labeled oligodeoxynucleotide or cDNA probes specific for $alpha$ -myosin heavy chain (MHC), $beta$ -MHC, atrial natriuretic factor (ANF), and sarco(endo)plasmic reticulum Ca²⁺-ATPase(SERCA) 2 mRNAs. To verify equal loading of the gel, the blot was also probed with an oligodeoxynucleotide probe specific for 18S rRNA. B: quantitative analysis of three Northern blotting experiments. The amounts of each transcript relative to the amount of 18S rRNA were quantified by scintillation spectroscopy and normalized to the relative mRNA levels in Adv-SR-infected NRVM. Data are means ± SE; *P < 0.05 by paired t-test.

Characterization of Adv-dnPKC- $epsilon$ . Next, we made use of an adenoviral vector encoding a dominant-negative mutant of PKC- $epsilon$ (Adv-dnPKC- $epsilon$ ; see Ref. 30). Thismutant form of PKC- $epsilon$ was generated by creating point mutationsin both the ATP-binding site and the pseudosubstrate domain. Themutations rendered the enzyme catalytically inactive while maintainingit in an active conformation, thereby enabling the mutated enzymeto localize to appropriate intracellularsites.

As seen in Fig. 4A, infection of NRVM with Adv-dnPKC- $epsilon$ resulted in a dose-dependent increase in PKC- $epsilon$ expression, as measuredby Western blotting of extractable total cell protein with monoclonalantibodies that recognized both endogenous and adenovirally expresseddnPKC- $epsilon$ . Viral concentrations in the range of 250-750 particles/cellproduced high levels of transgene expression. Subcellular fractionationrevealed that the majority of the immunoreactive PKC- $epsilon$ was foundin a Triton X-100 soluble membrane fraction of Adv-dnPKC- $epsilon$ overexpressingcells under basal conditions (Fig. 4B). In contrast, cells infectedwith Adv-SR showed that the majority of the endogenous enzymewas present in the cytosolic fraction. Stimulation of Adv-SR-infectedcells revealed the typical translocation of endogenous PKC- $epsilon$ fromthe cytosolic to the membrane (P₁) fraction within 10 min of ETtreatment. In contrast, there was no detectable increase in membrane-bound,immunoreactive PKC- $epsilon$ in ET-treated, Adv-dnPKC- $epsilon$ overexpressingcells. These results are consistent with the notion that overexpressionof dnPKC- $epsilon$ blocked translocation of the wild-type, endogenousPKC- $epsilon$ . However, translocation of the endogenous, wild-type PKC- $epsilon$ may have been masked by the abundant overexpression of "exogenous"dnPKC- $epsilon$ transgene. Therefore, endogenous PKC- $epsilon$ activity was measuredin the P₁ fraction of Adv-SR- and Adv-dnPKC- $epsilon$ -infected cells (Fig.4C). Membrane extracts from cells infected with Adv-SR showeda statistically significant 3.5 ± 0.9-fold increase in PKC- $epsilon$ activityin response to ET treatment for 10 min. Adv-dnPKC- $epsilon$ had no significanteffect on basal PKC- $epsilon$ activity compared with Adv-SR-infected cells.However, there was no ET-induced increase in PKC- $epsilon$ activity inthe membrane fraction of cells infected with Adv-dnPKC- $epsilon$ . Therewas also no significant difference in protein content of the membranefractions of the two groups of cells (200 ± 14 vs. 223 ± 25 µgprotein in the P₁ fraction of Adv-SR- and Adv-dnPKC- $epsilon$ -infectedcells, respectively; P = 0.45). Thus overexpression of dnPKC- $epsilon$ did not falsely "dilute" the active enzyme in the activity assay.Taken together, these data indicate that overexpression of highlevels of dnPKC- $epsilon$ indeed interfered with the translocation andactivation of endogenous, wild-type PKC- $epsilon$ .

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Fig. 4. Overexpression of dominant-negative (dn) PKC- $epsilon$ in NRVM. A: equal amounts (40 µg) of extracted cellular protein of uninfected cells and NRVM infected with increasing concentrations (50-1,000 ppc) of Adv-dnPKC- $epsilon$ were separated by SDS-PAGE. The resulting Western blot was then probed with a PKC- $epsilon$ -specific monoclonal antibody and visualized using an enhanced chemiluminensce technique. B: NRVM were infected with Adv-SR or Adv-dnPKC- $epsilon$ (750 ppc; 48 h). Cells were then stimulated with ET (100 nM, +ET) or diluent ( $-$ ET) for 10 min and subjected to subcellular fractionation. Equal amounts (40 µg) of extracted cellular protein from the cytosolic (Cyt) and Triton X-100-soluble membrane (P₁) fractions were separated by SDS-PAGE and Western blotting with a monoclonal antibody specific for PKC- $epsilon$ . C: PKC- $epsilon$ activity in similarly prepared P₁ fractions of unstimulated ( $-$ ET) and ET-stimulated (+ET) Adv-infected NRVM was measured using [³²P]ATP and a PKC- $epsilon$ -specific substrate peptide. Data (expressed as ³²P incorporated radioactivity) were normalized to the level of enzyme activity in the P₁ fraction of unstimulated, Adv-SR-infected NRVM. Data are means ± SE of 3-6 different subcellular fractionation experiments. *P < 0.05 vs. unstimulated cells by 1-way blocked ANOVA on Ranks followed by Student-Newman-Keuls test.

Activation of PKC- $epsilon$ is not necessary for ET-induced NRVM hypertrophy. We next examined whether PKC- $epsilon$ activation was necessary for the induction of cellular hypertrophy in response to ET. In theseexperiments, we compared the effects of ET treatment (100 nM,48 h) on cell surface area and total protein/DNA ratio in uninfectedcells, cells infected with the control Adv-SR, and NRVM infectedwith Adv-dnPKC- $epsilon$ . In the case of the uninfected cells, NRVM weretreated with ET for a total of 48 h. In the case of the Adv-infectedcells, ET treatment was begun 24 h after adenoviral infectionand continued for an additional 48 h. As seen in Fig. 5, ET resultedin a significant increase in cell surface area (Fig. 5A) and totalprotein/DNA ratio (Fig. 5B) in uninfected NRVM, which is consistentwith the ability of this peptide growth factor to induce cellularhypertrophy in low-density NRVM (5, 19, 23, 40). Infectionwith either Adv-SR or Adv-dnPKC- $epsilon$ had no significant effect oncell surface area or total protein/DNA ratio in unstimulated NRVM.As expected, ET significantly increased both indexes of NRVM hypertrophyin cells infected with Adv-SR, although the response was somewhatreduced compared with uninfected cells. Surprisingly, ET alsostimulated cell spreading and total protein accumulation in NRVMinfected with Adv-dnPKC- $epsilon$ . The response was virtually identicalto that observed in Adv-SR-infected myocytes.

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Fig. 5. Overexpression of dnPKC- $epsilon$ does not prevent ET-induced NRVM hypertrophy. A: NRVM were maintained under control conditions (uninfected) or infected with Adv-SR or Adv-dnPKC- $epsilon$ (750 ppc each). After 24 h, cells were then chronically stimulated with ET (100 nM, +ET) or diluent ( $-$ ET) for an additional 48 h. Cell surface area was then assessed by 2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein (BCECF) dye loading and image analysis. Data are means ± SE of 90-250 cells from each treatment group. *P < 0.05 vs. unstimulated cells in each group by Mann-Whitney Rank Sum test. B: total protein/DNA was assessed in similarly treated cultures. Data are means ± SE for 4-5 different cell isolations. *P < 0.05 vs. unstimulated cells in each group by paired t-test. C: total RNA was isolated from similarly treated NRVM. The resulting Northern blot was sequentially probed with ³²P-labeled oligodeoxynucleotide and cDNA probes specific for $alpha$ -MHC, $beta$ -MHC, ANF, and SERCA2 mRNAs and 18S rRNA.

We then examined whether PKC- $epsilon$ -dependent signaling was critical for the gene expression changes observed in ET-treated NRVM.Here too we compared the effects of ET on MHC, ANF, and SERCA2mRNA levels in uninfected cells, cells infected with the controlAdv-SR, and NRVM infected with Adv-dnPKC- $epsilon$ . As shown in Fig. 5C,adenoviral infection with either SR or Adv-dnPKC- $epsilon$ substantiallyreduced basal mRNA levels encoding $alpha$ -MHC and SERCA2 compared withuninfected NRVM. Other transcripts, such as $beta$ -MHC and ANF mRNAand 18S rRNA were less affected. ET treatment increased $beta$ -MHCand ANF mRNA levels three- to fivefold in uninfected NRVM whilesubstantially reducing $alpha$ -MHC and SERCA2 mRNA levels. ET treatmentreproduced the same "fetal" pattern of gene expression in Adv-SR-infectedcells, although the responses were somewhat blunted. Surprisingly,ET also stimulated this fetal gene program in NRVM infected withAdv-dnPKC- $epsilon$ . Again, the response was virtually identical to thatobserved in Adv-SR-infectedmyocytes.

Overexpression of dnPKC- $epsilon$ blocks ERK activation. In light of these somewhat unexpected findings, we examined whether dnPKC- $epsilon$ had any demonstrable effects on acute signalingevents in NRVM. Ping et al. (30) previously demonstrated thatinfection of cultured adult rabbit cardiomyocytes with Adv-dnPKC- $epsilon$ blocked ERK activation in response to simulated ischemic preconditioning,providing further evidence implicating PKC- $epsilon$ as an upstream regulatorof the ERK signaling cascade in cardiomyocytes. Because ET isa potent activator of ERK1/2 in NRVM (13) and AT-1 cardiac myocytes(24), we examined whether overexpression of dnPKC- $epsilon$ blockedERK1/2 activation in response to this hypertrophic agonist. Ofnote, we compared the effects of acute exposure to ET (100 nM,10 min) on ERK1/2 phosphorylation in NRVM infected with Adv-dnPKC- $epsilon$ vs. cells infected with the control Adv-SR. In both cases, acuteET stimulation was performed 24-48 h after adenoviral infectionto ensure high levels of dnPKC- $epsilon$ expression at the time of ETstimulation. As seen in Fig. 6A, ET increased ERK1/2 phosphorylationin Adv-SR-infected NRVM, as identified by Western blotting withan antibody that recognized only the phosphorylated forms of ERK1/2.In contrast, increasing concentrations of Adv-dnPKC- $epsilon$ markedlyreduced ET-induced ERK1/2 activation. These results were confirmedby gel-shift analysis, as depicted in Fig. 6B. As is evident fromthe Fig. 6B, ET induced an upward shift in the apparent molecularweight of both ERK1 and ERK2 in Adv-SR-infected NRVM. However,overexpression of dnPKC- $epsilon$ markedly suppressed this gel shift butdid not affect the total amount of ERK1 or ERK2 in the cells.Quantitative analysis of six separate phospho-ERK Western blottingexperiments is depicted in Fig. 6C. As is evident from Fig. 6C,basal levels of ERK2 phosphorylation were similar in Adv-SR- andAdv-dnPKC- $epsilon$ -infected NRVM. As expected, ET significantly increasedERK2 phosphorylation in Adv-SR-infected NRVM. However, ERK2 phosphorylationin ET-stimulated, Adv-dnPKC- $epsilon$ -infected NRVM was considerably reducedcompared with ET-stimulated, Adv-SR-infected cells (2.9 ± 0.6-vs. 1.6 ± 0.04-fold; P < 0.05). Nevertheless, dnPKC- $epsilon$ overexpressiondid not completely abrogate ERK2 phosphorylation. Furthermore,doubling the Adv-dnPKC- $epsilon$ concentration did not eliminate thisresidual ERK2 phosphorylation (see Fig. 6A), suggesting that PKC- $epsilon$ -independentpathways may play a role in regulating ERK2 phosphorylation inNRVM. Taken together, these data indicate that PKC- $epsilon$ is indeedupstream of the ERK cascade in cardiomyocytes but that acute activationof neither PKC- $epsilon$ nor ERK1/2 may be necessary for ET-induced proteinaccumulation, gene expression changes, and cellular growth.

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Fig. 6. Overexpression of dnPKC- $epsilon$ inhibits ET-induced ERK activation. A: NRVM were infected with Adv-SR (750 ppc) or Adv-dnPKC- $epsilon$ (100-1,500 ppc). After 24 h, cells were acutely stimulated with ET (100 nM, +ET) or diluent ( $-$ ET) for 10 min. Equal amounts of extracted cellular protein (40 µg) were then analyzed by SDS-PAGE and Western blotting with polyclonal antibodies that recognize only the active (phosphorylated) forms of extracellular signal-regulated kinase (ERK) 1 (p44) and ERK (p42) 2. B: similar cell extracts were separated by SDS-PAGE and Western blotting with polyclonal antibodies recognizing both active and inactive forms of ERK1 and ERK2. Activation is assessed by the presence of an upward band shift. C: quantitative results of 4-5 phospho (p)-ERK Western blotting experiments. Results were normalized to the band intensity of unstimulated, Adv-SR-infected cells. Data are means ± SE. *P < 0.05 vs. unstimulated cells by 1-way blocked ANOVA on Ranks followed by Student-Newman-Keuls test.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Our results indicate that caPKC- $epsilon$ overexpression in low-density NRVM was not sufficient to increase cell surface area or totalprotein/DNA ratio, although cell shape was altered markedly. Conversely,overexpression of dnPKC- $epsilon$ did not prevent NRVM hypertrophy inducedby the hypertrophic agonist ET but markedly suppressed ERK activation.These somewhat unexpected results suggest that PKC- $epsilon$ and downstreamsignaling via the ERK cascade are not necessary for the inductionof cardiomyocyte hypertrophy. It should be pointed out, however,that overexpression of mutant forms of PKC- $epsilon$ in NRVM maintainedin low-density culture may not be analogous to the activationof endogenous PKC- $epsilon$ in response to neurohormonal and mechanicalstimuli in the adult heart in vivo. First, PKC- $epsilon$ overexpressionwas accomplished under culture conditions in which NRVM displayno or only infrequent [Ca²⁺]_i transients and mechanical activity (18). These conditionsare quite distinct from the situation encountered in vivo, whereincardiomyocytes encounter both intrinsic and extrinsic mechanicalloading, display numerous cell-cell contacts, and continuouslycycle [Ca²⁺]_i. Second, the dnPKC- $epsilon$ studies used a mutant form of the rabbitenzyme to inhibit downstream signaling of the endogenous rat enzyme.Although dnPKC- $epsilon$ overexpression of the rabbit enzyme preventedET-induced increases in PKC- $epsilon$ activity in NRVM membranes, it isconceivable that, due to species differences, more subtle actionsof the endogenous enzyme were not prevented. Third, overexpressionof caPKC- $epsilon$ and dnPKC- $epsilon$ was accomplished by adenoviral infection.However, infection with high titers of Adv, even in the absenceof an inserted transgene, produced significant effects on cardiomyocytegene expression and partially suppressed ET-induced cell growth.Thus caution should be exercised in relating these studies tocardiomyocytes undergoing hypertrophy invivo.

Nevertheless, these cell culture results are interesting in light of recent studies that specifically examined the role ofPKC- $epsilon$ in cardiomyocyte growth and function in vivo. Takeishi etal. (43) and Mochly-Rosen et al. (28) recently described twodifferent transgenic mouse lines resulting in enhanced PKC- $epsilon$ -dependentsignaling. Both groups of animals demonstrated only mild concentricLVH with normal left ventricle function. $beta$ -MHC mRNA levels wereincreased in both studies, but other marker genes were less affected.In one of the lines, single cell capacitance, an index of cellvolume, was actually decreased, suggesting that the observed increasein left ventricle mass was actually the result of cellular hyperplasia,rather than an overall increase in the size of individual musclecells (28). Conversely, Khasar et al. (26) have describeda line of mutant mice lacking PKC- $epsilon$ . These animals have abnormalnociceptor regulation, increased sensitivity to acute behavioraleffects of ethanol (22), but normal cardiac development, andas adults they display no obvious cardiac phenotype. Taken together,these results and our own suggest that PKC- $epsilon$ may have a complexrole in overall growth regulation during cardiomyocyte hypertrophyandremodeling.

Despite its lack of effect on overall cell surface area, the shape of NRVM expressing caPKC- $epsilon$ was markedly affected. Thereis very little known about how cardiomyocytes convert mechanicaland neurohormonal signals into biochemical responses that inducealterations in cardiomyocyte shape. We were particularly interestedin whether the long, cell projections induced by caPKC- $epsilon$ overexpressioncontained actin filaments and whether these projections also containedfocal adhesions and/or costameres. Elegant studies by Dabiri andcoworkers (14) have indicated that myofibrillogenesis beginsat the cell surface by the organization of focal adhesion proteins,actin filaments, and nonsarcomeric myosin. As shown in Fig. 2,the elongated cell processes observed in Adv-caPKC- $epsilon$ -infectedNRVM indeed contained at least one focal adhesion component (paxillin),which was arranged in a striated pattern along F-actin filaments,consistent with the structural organization of focal adhesionsand costameres (19, 38). One can speculate that PKC- $epsilon$ mayin some way be involved in the regulation of sarcomeric assembly,especially at the ends of the growing myofibril. PKC- $epsilon$ has infact been localized by immunocytochemical techniques to regionsof the cell adjacent to or within costameres (7) and withinintercalated discs (17). Nevertheless, additional studies willbe required to further investigate the functional role of PKC- $epsilon$ in the assembly and maintenance of thesestructures.

In agreement with the transgenic overexpression studies described above, we found that adenovirally mediated caPKC- $epsilon$ overexpressionproduced selective alterations in NRVM gene expression. Our resultsconfirm previous findings of Decock et al. (15) who demonstratedthat overexpression of a constitutively active mutant of PKC- $epsilon$ increased ANF promoter activity. Of note, these investigatorsused transient, cotransfection of an ANF promoter-reporter geneconstruct along with the identical expression cassette used toconstruct the Adv-caPKC- $epsilon$ for the present report. Our resultsextend these findings by using an Adv to induce overexpression,rather than to rely on the relatively low transfection efficiencyprovided by the calcium phosphate precipitation method. Both cellculture studies indicate that caPKC- $epsilon$ overexpression was sufficientto increase ANF expression two- to threefold over control levels,which is contrary to that observed in the two transgenic linesdiscussed above (28, 43). In addition, we showed that mRNAlevels encoding $alpha$ - and $beta$ -MHC were markedly affected. caPKC- $epsilon$ overexpressionresulted in the typical MHC isoenzyme "switch" from $alpha$ - to $beta$ -MHCpredominance associated with contraction-induced (33, 34,36) and agonist-induced (23, 33, 46) NRVM hypertrophyin vitro and with pressure overload-induced cardiomyocyte hypertrophyin vivo (9). Interestingly, SERCA2 mRNA levels were unaffected,which is in agreement with both of the previously mentioned transgenicanimal experiments. It should be pointed out, however, that ANFand $beta$ -MHC mRNAs are readily detected in NRVM, even under basalconditions, in which cardiomyocytes display little or no spontaneous[Ca²⁺]_i and mechanical activity and have <5% of their total PKC- $epsilon$ inthe P₁ membrane fraction (41). Stimulation of [Ca²⁺]_i transients and contractile activity by membrane depolarizationin the absence of other factors was sufficient to translocatePKC- $delta$ , and to a much lesser extent PKC- $epsilon$ , and also to increaseANF and $beta$ -MHC promoter activities (41). Conversely, overexpressionof dnPKC- $epsilon$ (as described in the present report) markedly suppressedthe translocation of endogenous PKC- $epsilon$ into the membrane fractionbut failed to block the ET-induced alterations in ANF and MHCgene expression. Because ET increases [Ca²⁺]_i transients (19), and activates both PKC- $epsilon$ and PKC- $delta$ (13,31), there are likely to be other PKC- $epsilon$ -independent signalingpathways that regulate ANF and MHC gene expression in NRVM, evenunder conditions in which basal [Ca²⁺]_i transients and mechanical activity areminimized.

As demonstrated in Fig. 6, overexpression of dnPKC- $epsilon$ markedly suppressed ET-induced ERK activation, thus providing additional,strong evidence that PKC- $epsilon$ is an upstream regulator of the Ras-Raf-MEK-ERKcascade in cardiomyocytes (10, 13, 24, 29, 30). ERKsare acutely activated by a variety of neurohormonal agonists thatinduce NRVM hypertrophy, although their specific role in the inductionof various aspects of the hypertrophic phenotype remains controversial(1). Using adenovirally mediated overexpression of constitutivelyactive and dominant-negative mutants of MEK, Ueyama et al. (45)recently demonstrated that NRVM indeed utilize the ERK cascadeto induce hypertrophic responses, including upregulation of ANFgene expression. However, they indicated that interruption ofonly one pathway may be insufficient for complete inhibition ofthe hypertrophic responses induced by ET, PE, or mechanical stretch.Similarly, we recently showed that electrical stimulation of contractionincreased ANF and $beta$ -MHC promoter activity and induced NRVM hypertrophy,which was associated with the acute activation of Jun NH₂-terminalkinase (JNK) 2 and JNK3 but not ERK1 or ERK2 (41). Because ETacutely activates both JNKs (6, 12) and ERKs (4, 13,24), as well as PKC- $epsilon$ and PKC- $delta$ (4, 13, 24, 31), itseems reasonable to conclude that there is substantial cross talkbetween the novel PKCs and their downstream targets during hypertrophicsignaling. This conclusion is, of course, highly dependent onthe completeness of the block of PKC- $epsilon$ -dependent signaling byAdv-dnPKC- $epsilon$ overexpression. Furthermore, it should be pointedout that we were unable to completely abrogate ET-induced ERKactivation with the dominant-negative Adv. Thus it is conceivablethat the observed, residual level of ET-induced ERK phosphorylationwas sufficient to trigger the cell growth and gene expressionchanges observed in Fig. 5.

In summary, the results described in this report indicate that caPKC- $epsilon$ overexpression is sufficient to induce selective changesin cardiomyocyte gene expression indicative of the hypertrophicphenotype. Adv-caPKC- $epsilon$ altered cell geometry, producing cellularelongation and remodeling without a significant, overall increasein cell size or total protein accumulation. Furthermore, PKC- $epsilon$ activation and downstream signaling via the ERK cascade may notbe necessary for cell growth, protein accumulation, and gene expressionchanges induced by the hypertrophic agonist ET-1. Future studieswill be necessary to determine whether the other PKC isoenzymesexpressed in cardiomyocytes are necessary and/or sufficient aloneor in combination to induce specific aspects of this complexphenotype.

	ACKNOWLEDGEMENTS

We thank Alan G. Ferguson and Beverly Martin for excellent technical assistance and Drs. Peter Parker, Peter Sugden, and PeipeiPing for the provision of valuablereagents.

	FOOTNOTES

This work was supported in part by National Heart, Lung, and Blood Institute Grants RO1 HL-34328 and RO1 HL-63711 and a giftto the Cardiovascular Institute from the Dr. Ralph and MarianFalk Trust for Medical Research. J. B. Strait was supported inpart by a Loyola University Chicago Dissertation Fellowship, andD. M. Eble was supported in part by a Beck/Scanlon CardiovascularResearch Development Award during the time these studies wereperformed.

Address for reprint requests and other correspondence: A. M. Samarel, The Cardiovascular Institute, Bldg. 110, Rm. 5222, LoyolaUniv. Medical Center, 2160 South First Ave., Maywood, Illinois60153 (E-mail: asamare{at}lumc.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 18 July 2000; accepted in final form 2 October 2000.

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Role of protein kinase C- in hypertrophy of cultured neonatal rat ventricular myocytes

Role of protein kinase C- $epsilon$ in hypertrophy of cultured neonatal rat ventricular myocytes