Changes in protein kinase C in early cardiomyopathy and in gracilis muscle in the BB/Wor diabetic rat

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Changes in protein kinase C in early cardiomyopathy and in gracilis muscle in the BB/Wor diabetic rat

Thomas D. Giles, Jie Ouyang, E. Kenneth Kerut, Michael B. Given, Gayle Eileen Allen, Elizabeth F. McIlwain, and Stan S. Greenberg

Department of Medicine, Section of Cardiology, Cardiovascular Research Laboratories, and Department of Physiology, Alcohol Research Center, Louisiana State University Medical Center, New Orleans, Louisiana 70112

ABSTRACT

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Abstract
Introduction
Materials
Results
Discussion
References

Hyperglycemia can upregulate protein kinase C (PKC), which may be an important mediator of the progression from normal heartand muscle function to diabetic myopathy in the myocardium andskeletal muscle in type 1 insulin-dependent diabetes mellitus(IDM). We evaluated this possibility during the early stage ofIDM in BB/Wor diabetic (D) rats and age-matched BB/Wor diabetes-resistant(DR) rats. Interventricular septal thickness, E wave peak velocityof tricuspid inflow (both minimum and maximum), and left ventricular(LV) weight index were increased, and the rate of change in LVpressure (LV dP/dt) decreased in D rats subjected to M-mode andtwo-dimensional echocardiography and hemodynamic recording ofheart rate, LV pressure (LVP), +LV dP/dt, $-$ LV dP/dt, and LV end-diastolicpressure (LVEDP) in vivo and in vitro 41 days after the onsetof hyperglycemia. Whole ventricle basal PKC activity was increasedby 44.4 and 18.4% in the particulate and soluble fractions, respectively,from D rats compared with that from DR rats using r-³²P phosphorylation of appropriate peptide substrates. When measuredby Western blot gel densitometry, particulate PKC- $alpha$ and PKC- $delta$ content increased by 89 and 24%, respectively, but soluble PKC- $beta$ and soluble and particulate PKC- $epsilon$ were unchanged compared withthat of DR rats. Similarly, gracilis muscle PKC activity and PKC- $alpha$ and PKC- $delta$ were elevated in the gracilis muscle, whereas that ofthe circulating neutrophil did not differ between the D and DRrats. Thus, in vivo, the early diabetic cardiomyopathy of theD rat is characterized by a restrictive LV with increased septalthickness and is associated with elevated PKC activity and increasedamounts of myocardial particulate PKC- $alpha$ and PKC- $delta$ , which are alsoseen in the skeletal muscle. We conclude that increased PKC isozymesmay play a pivotal role during IDM in the development of diabeticcardiomyopathy and skeletal muscle myopathy.

echocardiography; genetic diabetes; Doppler flowmetry; protein kinase C isozymes; myocardial contractility

	INTRODUCTION

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IN HUMANS type 1 insulin-dependent diabetes mellitus (IDM) is associated with the development of cardiomyopathy, which isindependent of the myocardial disease produced by coronary atherosclerosis(13, 15, 38, 44). Diabetic cardiomyopathy appears to beresponsible for some of the excess cardiovascular morbidity andmortality that occurs in diabetic patients (14, 38, 44).Many biochemical and metabolic defects have been observed in themyocardium and skeletal muscle of animals and patients with IDMas well as type 2 diabetes, including diabetic cardiomyopathy,increased $beta$ -myosin heavy chain ( $beta$ -MHC) and ventricular myosinlight chain 2 (vMLC-2), impaired Ca²⁺-activated actinomyosin adenosinetriphosphatase (ATPase) activityof the ventricular myocytes, increased secretion of atrial natriureticpeptide (ANF) and angiotensin II-converting enzyme (ACE), skeletalmuscle weakness, impaired utilization of glycogen stores and glucosein skeletal muscle, and a decrease in the number of glucose transporters(GLUT-4) in skeletal muscle membranes (4, 6, 38, 44).Nevertheless, the basic biochemical and molecular biological defectsresponsible for the transformation of normal to diseased myocardiumand skeletal muscle remain undefined (2, 13, 14, 38,44). Recent studies suggest that IDM may result from an overactiveimmune response of T-lymphocytes and macrophages, which invadethe $beta$ -pancreatic cells and release cytokines and free radicals,including nitric oxide, which then destroy these cells, impairingtheir ability to manufacture and secrete insulin (4, 6,7, 29). This concept was based on the findings in the BB/Worrat and NOD mouse, which develop IDM similar to that seen in humansand in which cyclosporin, an immunosuppressant, can prevent theonset of diabetes (4, 6, 29). However, human clinicaltrials with cyclosporin have met with only limited success becauseof the nephrotoxicity of this drug and the severity of the pancreaticdamage at the time of diagnosis of IDM in humans (4, 29).Thus the BB/Wor diabetic rat can be used as a model for humantype 1 IDM-mediated cardiomyopathy and skeletal muscle myopathy.

Protein kinase C (PKC) is a family of enzymes involved in the phosphorylation of enzymatic and regulatory protein substrates(21, 23). Phosphorylation and dephosphorylation of enzymesare important physiological mechanisms utilized for the activationand deactivation of enzymatic activity (15, 21, 23). Twelveisozymes of PKC have been identified and subsequently subdividedinto three major categories: 1) Ca²⁺-dependent and phospholipid- and diacylglycerol (DAG)-activatedPKC isozymes (cPKC), 2) Ca²⁺-independent and phospholipid- and DAG-activated PKC (nPKC), and3) atypical PKC isozymes (aPKC) that are Ca²⁺ independent and activated by phosphatidylcholine or phosphatidylethanolamine(15, 21, 23, 36). Activation of PKC may result from mechanicaland physical deformation of the myocardial cell membrane (e.g.,stretching or distension), the interaction of agonists with theirmyocardial cell membrane receptors, or elevated intracellularconcentrations of the substrates that activate PKC, includingDAG, phosphatidylcholine, phosphatidylethanolamine, and Ca²⁺. Mechanical distension or the inter- action of agonists withtheir myocardial membrane receptors activates phospholipase C,resulting in the hydrolysis of phosphatidyl 4,5-bisphosphate intoinositol (1,4,5)-trisphosphate [Ins(1,4,5)P₃] and DAG. Ins(1,4,5)P₃releases intracellular Ca²⁺, which then combines with cytosolic cPKC. This aids in the bindingof an inactive form of cPKC to the phosphatidylserine (PS) residuesof the cell membrane. The binding of DAG to the membrane-boundinactive form of cPKC results in its activation and subsequentability to phosphorylate enzymes or receptor proteins. Alternatively,DAG can bind to inactive nPKC. This allows the binding of theDAG-nPKC complex to PS residues in the membrane and results inthe subsequent activation of nPKC (15, 21, 23, 36). Analternate pathway for activation of PKC also exists. Activationof phospholipase D hydrolyzes phosphatidylcholine to phosphatidicacid, which is further metabolized to DAG and to phosphatidylethanol.Both DAG and phosphatidylethanol can subsequently activate PKC(15, 21, 36). A similar mechanism exists in skeletal muscle(15, 23, 36).

Phosphorylation of myocardial and skeletal muscle enzymes and proteins by PKC isozymes can affect cardiac rhythm and cardiacand skeletal muscle contractility, gene expression, and growth(2, 12, 15-17, 21, 23, 24, 35, 36, 40, 42).Protein kinase C-mediated phosphorylation of troponin T, troponinI, troponin-tropomyosin complex, and troponin-C protein in isolatedmyocardial and skeletal muscle cells is associated with inhibitionof Ca²⁺-activated myofibrillar actomyosin MgATPase activity and contractility(21, 23, 24). The PKC- $delta$ isozyme can increase Ca²⁺ influx through L-type Ca²⁺ channels (35), which are also present in the membrane of ventricularmyocytes and skeletal muscle (15, 21, 23, 29). Activationof cPKC- $delta$ and nPKC- $epsilon$ is associated with myocardial ventricularhypertrophy, including overexpression of $beta$ -MHC, vMLC-2, ANF, andACE (36).

Recent studies in vascular smooth muscle and in cardiac myocytes in culture suggest that elevated plasma levels of glucose,the hallmark of both type 1 and type 2 diabetes mellitus, maybe causal to elevated tissue levels of PKC and thereby may playa pivotal role as a mediator of the progression from normal todiseased vasculature and myocardium (1, 8, 16, 25, 26,39, 42). Hyperglycemia may increase the DAG content of therat myocardium (16, 25, 26). Total PKC activity also increasedin the myocardium of diabetic rats (37, 43). Persistent upregulationof PKC activity may lead to alterations in myocardial contractilityand cell growth (2, 13, 15-17, 21, 24, 25, 36, 37,40, 42), which may compensate for the potential decrease ofprotein synthesis resulting from impaired sensitivity of the diabeticmyocardium to this action of adenosine 3',5'-cyclic monophosphate(cAMP) (32). Moreover, sustained elevations of PKC activitycan increase the activity of serum and tissue levels of ACE inthe diabetic rat (39).

Increased ACE activity can increase sera and tissue levels of angiotensin II, which can cause myocardial remodeling and hypertrophy(35, 38). We previously reported that treatment of rats withthe ACE inhibitor benazepril prevented the development of myocardialdysfunction in streptozocin (STZ)-induced diabetic cardiomyopathy(9). These data all suggest that dysregulation of PKC may playa pivotal role in the development of cardiac and skeletal musclemyopathy in IDM. However, if changes in PKC are causal to thedevelopment of diabetic myopathy, we hypothesize that alterationsin PKC must be present early in its development at a time whenfunctional abnormalities would be minimal or absent. We testedthis hypothesis in BB/Wor diabetic (D) and diabetic-resistant(DR) rats by measurement of the activity and total quantity ofPKC and PKC isozymes in ventricular tissue, gracilis muscle, andcirculating neutrophils and by measurement of cardiac structureand function in vivo, using hemodynamic measurements and echocardiography,and direct evaluation of myocardial function in vitro, utilizingthe isolated working heart preparation.

	METHODS AND MATERIALS

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General experimental protocol. Male BB/Wor D rats (diabetic for 30-41 days) and age-matched DR rats were obtained from the National Institute of Diabetesand Digestive and Kidney Diseases breeding and maintenance facilityat the University of Massachusetts. The D rats were maintainedon daily subcutaneous injections of 0.6-3.0 U/rat of a long-acting(once a day) protamine, zinc, and insulin suspension (protamine,zinc, and Iletin I, Eli Lilly, Indianapolis, IN) before theirfeeding period on the basis of their urinary excretion of glucosefrom the first appearance of glucosuria. DR rats were given equivalentsubcutaneous injections of vehicle. Daily injections of insulinwere necessary because the D rats, a model for IDM, die withina few days without insulin maintenance. All animals were housedon a 12:12-h light-dark cycle with access to water and standardrat chow ad libitum. All animals were anesthetized intramuscularlywith a solution consisting of (in mg/kg) 50 ketamine-4 xylazinebefore echocardiography and Doppler flowmetry or surgery for collectionand measurement of blood for serum glucose concentrations usinga standard glucose monitor (Boehringer Ingelheim, Ridgefield,CT). The D and DR rats were subdivided into two cohorts. One cohortwas subjected to echocardiography and Doppler flowmetry followedby invasive measurement of cardiovascular dynamics. Their bloodwas removed and the neutrophils were isolated on a Ficoll-Percollgradient as described previously (20). The hearts were alsoremoved and the ventricles were rapidly frozen in liquid nitrogen.The second cohort of rats was subjected to echocardiography andDoppler flowmetry and the hearts were then removed and used forin vitro perfusion while the gracilis muscle was removed and frozenin liquid nitrogen. The ventricles, gracilis muscles, and neutrophilswere assayed for PKC activity and isozyme content as describedbelow. The experimental protocol (1224) was approved by the LouisianaState University Institutional Animal Care and Use Committee.

Echocardiographic analysis of cardiac performance. M-mode and two-dimensional echocardiograph and Doppler flow recordings were made using a Toshiba model 270 echocardiographyinstrument with a 7-MHz transducer. The transducer was calibratedwith phantoms before use. Two-dimensional echocardiograms wererecorded from both parasternal long- and short-axis views, apicalfour-chamber views and suprasternal views of the aortic valve,and from both ascending and descending aorta. M-mode recordingswere obtained of the left ventricle (LV) at the level of the mitralpapillary muscle and at the level of the mitral valve in the parasternalview using two-dimensional echocardiographic guidance in boththe short- and long-axis views. Aortic valve M-mode recordingsfrom the parasternal long-axis and suprasternal views were obtained.Pulsed-wave Doppler was used to examine mitral diastolic inflowfrom the apical four-chamber view and tricuspid diastolic inflowfrom the apical four-chamber and parasternal short-axis views.Aortic valve flow and isovolumic relaxation time were calculatedfrom the apical five-chamber view using pulsed-wave Doppler. ColorDoppler studies were performed for evaluation of LV length fromthe apical four-chamber view. Color-flow imaging was also usedto determine flow in both ascending and descending aorta fromthe suprasternal view. Data were recorded on Super VHS 0.5-in.tape for playback. Six consecutive cardiac cycles for each viewand parameter were digitized from tape onto a Freeland digitalacquisition system, and the average value was calculated. Echocardiographicmeasurements included M-mode interventricular septal thickness,LV internal dimension at the end of diastole, and M-mode posteriorLV wall thickness using the leading edge-leading edge method asrecommended by the American Society of Echocardiography (22).Mitral Doppler peak E and A wave velocities and E:A ratio, tricuspidDoppler E and A wave velocities and E:A ratio (both minimum andmaximum), and the difference between maximum and minimum E waveDoppler velocities ( $Delta$ E Vel_maxmin) were obtained. Tricuspid $Delta$ E Vel_maxmin was also calculated.

Determination of LV performance in vivo. The anesthetized rats were placed on a blanketed, temperature-controlled surgical table (37°C). A polyethylene catheter (PE-30)connected to a Gould P23D pressure transducer was advanced intothe LV via the right carotid artery. The position of the catheterin the LV was confirmed by the LV pressure (LVP) tracing. AfterLVP and heart rate (HR) stabilized, HR, LVP, and the positiveand negative rate of change of LVP (+LV dP/dt and $-$ LV dP/dt) werecontinuously recorded and continuously logged on an Apple 650Quadra computer. The data for 1-min increments were obtained at300 Hz, and the average values were calculated. +LV dP/dt and $-$ LV dP/dt were obtained by differentiation of the LVP signals.

Determination of cardiac performance in vitro. Hearts were perfused on a standard working heart apparatus as described previously in detail (9). Heparin sodium (200 Uiv) was administered to the rats immediately before they werekilled, and 50 U/ml were added to the initial perfusate, Krebs-Henseleitbuffer aerated with a 95% O₂-5% CO₂ mixture, to maintain a pHof 7.4. The perfusate was filtered using a Whatman Polycap HDfilter (10-µm pore size) to prevent cells and debris from cloggingthe coronary circulation. All hearts were paced at 250 beats/minand allowed to stabilize before the start of the experiment. Aorticpressure, measured with a Statham P23Db transducer positionedat the level of the aortic valve, was set at 65 mmHg. LVP wasmeasured with a Statham P23Db pressure transducer connected toa 26-gauge needle inserted through the ventricular wall at the"dimple" located at the apex of the heart. The LVP transducerwas positioned at a level corresponding to midventricle. Positiveand negative LV dP/dt were obtained by differentiating the LVPsignal. Left atrial pressure (LAP) was measured via an atrialcannula connected to a Statham P23Db pressure transducer positionedat the level of the left atrium and was varied during the experimentby adjusting the height of the atrial reservoir. Initial LAP wasset at 10 cmH₂O. After equilibration of the heart, LAP was reducedto 5 cmH₂O, increased in 5-cmH₂O increments to a maximum of 20cmH₂O, and then reduced to 10 cmH₂O at the end of the experiment.The response of the heart to each increase in LAP was allowedto stabilize before the recording of the data. Pressures and derivedindexes were recorded on a Grass model 79 polygraph. An AppleMacintosh Quadra 650 computer sampled and digitized the data fromthe polygraph for storage and subsequent analysis. The cardiacperformance parameters measured were maximum developed LVP (LVP_max),+LV dP/dt, $-$ LV dP/dt, and LAP.

Specificity of assay for PKC isozymes. Recent data suggest the possibility that some antibodies specific for PKC isozymes cross-react with other PKC isozymes togive false indexes of the identity and quantity of PKC isozymepresent in various tissues (30). To ascertain the existenceor absence of constitutive PKC isozymes and the specificity ofthe antibodies used to test for the presence of the PKC antibody-specificproteins, we analyzed the ventricular homogenate for the presenceof PKC isozyme mRNA and protein and subsequently performed PKCantibody isozyme neutralization using authentic PKC isozyme peptidesas antigens.

Determination of cDNA for PKC isozymes. Transcripts for PKC isozymes were measured by reverse transcriptase-polymerase chain reaction (RT-PCR) in whole homogenatesof ventricular myocardium as previously described for alveolarmacrophages (10, 11, 20). Briefly, the total RNA of thehomogenized ventricle was isolated using Trizol reagent (GIBCO,Gaithersburg, MD). Total cDNA was obtained by reverse transcriptionof total RNA and was labeled with [³²P]dCTP. Total cDNA (10 ng) was amplified by using the specificPKC isozyme primers and [³²P]dCTP. Primer sequences for the PKC isozymes are shown in Table1. The relative amounts of PKC isozyme cDNA were determined byphosphorimager scan and quantitation of the smear and signal bands,normalized to that of $beta$ -actin (n = 8) as described previouslyin detail (10, 11, 20). Whole homogenate PKC isozyme contentwas determined with Western blot analyses.

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Table 1. Primer sequence and base pair of PKC isoforms

Western blot analyses of PKC isozymes. Western blot analyses were performed as described previously for the assay of nitric oxide synthase protein (10, 11) butwere modified for the myocardium and gracilis muscle and for extractionand detection of PKC isozymes. Aliquots of frozen ventricle, gracilismuscle, or neutrophils obtained from BB/Wor homozygous D and DRrats were quantitatively pulverized and homogenized in homogenizationbuffer I [20 mM tris(hydroxymethyl)aminomethane (Tris) · HCl,pH 7.5, 0.25 M sucrose, 2 mM EDTA, 2 mM ethylene glycol-bis( $beta$ -aminoethylether)-N,N,N',N'-tetraacetic acid (EGTA), 0.02% leupeptin, 1 mMphenylmethylsulfonyl fluoride (PMSF), and 0.1% Triton X-100] ina cold room. The homogenates were incubated for 1 h at 4°C andsubsequently centrifuged (17,500 g for 30 min at 4°C). The supernatantswere then centrifuged at 37,000 g to isolate the mitochondria,the resulting supernatant was centrifuged at 100,000 g at 4°C,and the particulate (membrane) and soluble fractions (cytosol)were stored at $-$ 20°C until assayed for protein with the bicinchoninicacid (BCA) method (10, 11). The protein samples (50 or 100µg) were then separated by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) using a 10% (wt/vol) acrylamideseparating gel and a 4% (wt/vol) acrylamide stacking gel. Theprotein was then electrophoretically transferred to nitrocelluloseusing a Semi-Dry transfer cell (Bio-Rad, Hercules, CA) and a transferbuffer consisting of Tris · HCl (48 mM) and 39 mM glycine (pH9.2) containing 0.037% (wt/vol) SDS and 20% (vol/vol) methanol.

After nonspecific sites were blocked with blocking solution [phosphate-buffered saline (PBS) without heparin, containing 5%(wt/vol) nonfat milk and 0.05% (vol/vol) Tween-20] for 1 h atroom temperature, the nitrocellulose was incubated with the primaryantibodies (GIBCO BRL, Grand Island, NY; Transduction Laboratories,Lexington, KY) in buffer II [1/1,000 to 1/2,000 dilution in PBSwithout heparin, containing 1% (wt/vol) nonfat milk and 0.05%(vol/vol) Tween-20] overnight at 4°C. The nitrocellulose was thenwashed three times, for 10 min each, with blocking buffer devoidof nonfat milk and then incubated at room temperature for 1 hwith horseradish peroxidase-linked secondary antibody (1/5,000dilution in buffer II ). After an additional series of three 10-minwashes in blocking solution devoid of nonfat milk, the bound antibodyon the filter was detected by the enhanced chemiluminescence method,according to the manufacturer's instructions (Amersham-Searle,Arlington Heights, IL). Exposure times of immunoblots to Hyperfilmwere 1-60 min and were identical for samples obtained from DRand D rats. Semiquantitation of PKC isozymes was performed bydensitometric analysis of the autoradiographs using NIH-IMAGEand a Logitech-3+ scanner (Logitech, Fremont, CA) on a MicronPentium 133 computer (Microsystems, New Orleans, LA). Particulateand soluble ventricle, gracilis muscle, and neutrophil PKC isozymeand the relative distribution of isozyme among the soluble andparticulate fractions were determined by gel densitometric analysisof the PKC isozyme/50 µg of protein, expressed as a product ofthe total protein in each fraction. Data were expressed as geldensity units per 50 µg of protein corrected for the gel densityunits of 50 µg of albumin or as a percentage of the PKC isozymecontent of an equivalent amount of protein obtained from the ventricular,gracilis muscle, or neutrophil fraction of the DR rat, respectively,analyzed simultaneously.

Determination of specificity of antibodies for PKC isozymes. Protein extracts (50 and 100 µg) of ventricular myocardium prepared as described in Determination of cDNA for PKC isozymeswere subjected to SDS-PAGE electrophoresis as described in Westernblot analyses of PKC isozymes. Immunoblots were prepared as describedin Western blot analyses of PKC isozymes with PKC isozyme-selectiveantibodies (0.5 µg/ml) that had been preincubated (+) or had notbeen preincubated ( $-$ ) with the isozyme-specific antigen peptide(1 µg/ml), which was used as a specific antibody antagonist (TransductionLaboratories). The PKC isozyme-specific antibody that is preincubatedwith its corresponding antigen peptide should lose its abilityto bind to the antibody-selective PKC isozyme because its bindingsites should now be occupied by the antigen peptide. If a signalband was selectively blocked by incubation of the antibody withthe corresponding antigen peptide, it was defined as a specificsignal that contained the same structure as the correspondingantigen peptide.

Measurement of PKC activity. Ventricles, gracilis muscle, and neutrophils were rapidly removed from the D and DR rats utilized in the in vivo studies describedin Determination of LV performance in vivo. The pieces of tissuewere washed in PBS to remove residual blood and were then frozenin liquid nitrogen. Portions of the frozen ventricles, gracilismuscle, and neutrophils were quantitatively pulverized and thenplaced in homogenization buffer I (20 mM Tris · HCl, pH 7.5, 0.25M sucrose, 2 mM EDTA, 2 mM EGTA, 0.02% leupeptin, and 1 mM PMSF)and homogenized in a cold room with a Polytron set at 7 for 20s, followed by homogenization for 60 strokes using a Dounce homogenizer.The homogenates were centrifuged as described in Western blotanalyses of PKC isozymes for the PKC isozyme assay, and the particulateand soluble fractions were obtained for measurement of PKC activity.The pellets were washed and resuspended in buffer II (20 mM Tris· HCl, pH 7.5, 2 mM EDTA, 2 mM EGTA, 0.02% leupeptin, 1 mM PMSF,and 0.1% Triton X-100) and again homogenized. The homogenateswere solubilized in buffer II without Triton X-100. After a 45-minincubation period at 4°C, the soluble fraction was obtained byultracentrifugation at 100,000 g for 30 min, and the pellet wasretained as the particulate or membrane fraction. Both membraneand soluble fractions were passed through 0.5 ml DEAE columns(Pharmacia, Gaithersburg, MD), washed twice with buffer II (2ml), and then eluted with 0.4 ml of phosphate buffer containing200 mM NaCl (37). PKC activity was determined with an Amershamkit for PKC activity (Amersham, Arlington Heights, IL) by measurementof the phosphorylation of the specific substrate octapeptide (RKRTLRRL)in the presence of Ca²⁺, PS, and DAG using [³²P]ATP. (Amersham Searle, Waltham, MA). The protein content ofthe fractions was measured by the BCA method as described previouslyin detail (10, 11). The enzymatic data were expressed as picomolesper milligram protein per minute after comparison to a standardcurve and correction for the nonspecific kinase activities foundin the absence of Ca²⁺, PS, and DAG.

Statistical analysis of data. Each experiment contained four to six animals per treatment group. Data were analyzed with analysis of variance (ANOVA) fora randomized complete block or completely random sample design.Differences between and among means were analyzed with Dunnett'sand Duncan's tests. Biochemical data were analyzed with multipleANOVA and means were compared with Newman-Keuls test; P < 0.05was accepted for statistical differences between and among means.

	RESULTS

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Body weights, blood glucose concentration, and cardiac measurements. Body weights did not differ among the DR and D rats (Table 2). The D rats demonstrated glucosuria between 28 and 49 daysafter their birth and were diabetic, as evidenced by a glucosuriaof +2 to +4, for 6-8 wk before they were killed. At the time ofdeath blood glucose concentrations were increased in D rats comparedwith those of DR rats (P < 0.05) (Table 2). Although total heartweight and LV mass did not differ among the DR and D rats, therewas a small but insignificant increase in LV mass (P = 0.076)and a significant increase in LV mass index (LV wt/body wt; P= 0.013) in the LV obtained from the BB/Wor D rats compared withthe LV mass index obtained from the DR rats. When total heartweight was expressed as a percentage of total body weight (heartweight index), no significant difference was observed betweenDR and D rats (Table 2). Interventricular septal weight was increasedin the hearts obtained from the BB/Wor D rats compared with thatobtained from the DR rats (P = 0.03).

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Table 2. Comparison of body weight, blood glucose, and cardiac weight of BB/Wor DR rats and BB/Wor rats

Echocardiographic measurements. Analysis of M-mode echocardiographic recordings revealed an increase in interventricular septal thickness in D rats comparedwith that obtained from DR rats (P = 0.05), whereas no significantdifference in LV internal dimension or LV posterior wall thicknesswas evident between the two groups of rats (Table 3). Dopplerpatterns of mitral inflow did not differ between the DR and Drats. However, the E wave peak velocity of tricuspid inflow (bothminimum and maximum) was increased in the D rats compared withthat of the DR rats (P = 0.03) (Table 3, Fig. 1).

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Table 3. M-mode echocardiographic and Doppler flowmetry analyses of hearts from BB/Wor DR rats and BB/Wor D rats

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Fig. 1. Typical echocardiogram showing increased tricuspid E wave and decreased A wave velocities in the BB/Wor diabetic (D) rat (A) and diabetes-resistant (DR) rat (B).

Determination of LV performance in vivo and in vitro. LVP_max did not differ between the BB/Wor DR and D rats (Table 4). Moreover, LVEDP was not significantly elevated in the Drats compared with that of the DR rats (Table 4). In contrast,myocardial contractility as reflected by +LV dP/dt (P < 0.05)and the rate of relaxation of the LV as reflected by $-$ LV dP/dt(P = 0.08) were lower in the BB/Wor D rats compared with theseparameters in the BB/Wor DR rats (Table 4). However, no significantdifferences in myocardial function existed in vitro in the paced,isolated hearts obtained from the D and DR rats when maintainedat an LAP of 5 or 20 cmH₂O (data not shown) and at 10 cmH₂O (Table4).

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Table 4. In vivo and in vitro cardiac function of BB/Wor DR and BB/Wor D Rats

PKC isozyme mRNA, specificity of antibody, and linearity of PKC isozyme content and enzymatic activity. The constitutive mRNAs present in the ventricle of the D rats as determined by RT-PCR were PKC- $delta$ >>> PKC- $epsilon$ > PKC- $alpha$ > PKC- $gamma$ = PKC- $zeta$ >>> PKC- $beta$ (Fig. 2). Similarly, the PKC isozymes detectablein the whole homogenate of ventricle were PKC- $delta$ >> PKC- $epsilon$ = PKC- $alpha$ (Fig. 3). When the ventricular homogenate was separated into thesoluble (cytosolic) and particulate (membrane) fractions, thePKC isozymes detectable in the membrane fraction of the ventriclewere PKC- $delta$ >> PKC- $epsilon$ = PKC- $alpha$ , whereas those of the cytosol werePKC- $alpha$ > PKC- $epsilon$ > PKC- $delta$ > PKC- $zeta$ > PKC- $beta$ > PKC- $gamma$ . PKC- $beta$ and PKC- $gamma$ were absent in two of five ventricles despite the presence oftheir mRNA (Fig. 3). Each of the PKC isozyme-specific antibodieselicited a signal when reacted with its authentic isozyme andwith the brain extract at a molecular weight that correspondedto the authentic PKC isozyme. PKC- $zeta$ was detectable in the cytoplasmof the unstimulated ventricle, PKC- $beta$ and PKC- $gamma$ were barely detectablein the cytoplasm of the adult rat ventricle, and PKC- $alpha$ , PKC- $epsilon$ ,and PKC- $delta$ were found in both the cytoplasm and membrane extractsof the adult rat ventricle. Because the antibodies for PKC- $beta$ ,PKC- $gamma$ , and PKC- $zeta$ failed to give any significant signal in therange of 72 to 90 kDa in the particulate fraction that containedsignificant amounts of PKC- $delta$ and PKC- $epsilon$ , it is unlikely that anysignificant cross-reactivity existed between these antibodiesfor PKC isozymes and PKC- $delta$ and PKC- $epsilon$ . Moreover, because PKC- $delta$ and PKC- $epsilon$ did not give any signals at the molecular weight ofeach other, it is also unlikely that cross-reactivity exists betweenthese isozymes. Finally, preincubation of the PKC isozyme-specificantibodies with their antigen-specific proteins eliminated thedetection of a band at the corresponding molecular weight of theantibody-specific isozyme (Fig. 3). Similar results were obtainedin the skeletal muscle extracts (data not shown). Thus, underthe conditions of the experiment and with these tissues, the antibodiesused appeared to be isozyme specific.

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Fig. 2. Typical reverse transcriptase-polymerase chain reaction (RT-PCR) gel of protein kinase C (PKC) mRNA (A) and Western blot of particulate protein of PKC isoforms (B) found in ventricle of adult D rat. A: $alpha$ , $beta$ , $gamma$ , $delta$ , $epsilon$ , $eta$ , and $zeta$ indicate PKC isozyme cDNA that is being tested; M column represents no. of base pairs (bp). Bottom bands in A represent those of $beta$ -actin. Constitutive PKC isozyme mRNAs present in DR rat ventricles are PKC- $delta$ >>> PKC- $epsilon$ > PKC- $alpha$ > PKC- $gamma$ = PKC- $zeta$ . For details, see METHODS AND MATERIALS.

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Fig. 3. Effect of antigen-specific neutralization of PKC isozyme antibodies on detection of PKC isozymes by Western blot in homogenates of rat brain and in cytosolic and membrane fractions of rat heart (H). $-$ , PKC isozyme was detected in presence of antibody alone; +, PKC isozyme was tested for with antibody preincubated with specific antigen peptide. In this animal PKC- $beta$ and PKC- $gamma$ isozymes are barely detectable. Note the absence of any significant signals after antigen-specific antibody neutralization (for details, see METHODS AND MATERIALS).

The gel density units of each of the isoforms of PKC- $alpha$ , PKC- $beta$ II, PKC- $delta$ , PKC- $gamma$ , and PKC- $epsilon$ in the soluble fraction and PKC- $alpha$ ,PKC- $delta$ , and PKC- $epsilon$ in the particulate fraction of the ventriclewere linearly related to the amount of protein applied to thegels (Fig. 4). PKC- $beta$ II and PKC- $gamma$ were absent in the particulatefraction of the ventricle (Fig. 4). Finally, the enzymatic activityof PKC present in total homogenates and the particulate and solublefractions of the ventricles obtained from DR rats were also dependenton the amount of protein used in the assay (Fig. 5). Similar resultswere obtained with the neutrophil and skeletal muscle (data notshown).

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Fig. 4. Relationship between optical density (gel density units/mm²) of Western blot of PKC isozymes as a function of protein applied to gels in ventricles obtained from D rat. A: soluble fraction. B: particulate fraction. Each mean value represents n = 5 rats.

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Fig. 5. PKC activity of particulate, soluble, and total homogenate of ventricle expressed as function of amount of ventricular protein used in assay (pg of substrate/20 min). For details, see METHODS AND MATERIALS. Each mean and SD represent responses from 5 animals.

Ventricular PKC isozyme content and PKC activity. PKC- $alpha$ , PKC- $beta$ , PKC- $delta$ , and PKC- $epsilon$ were the predominant PKC isozymes in the soluble fraction of the rat heart, with PKC- $alpha$ andPKC- $delta$ in most abundance (Figs. 6 and 7). In contrast, PKC- $alpha$ , PKC- $delta$ ,and PKC- $epsilon$ were the only PKC isozymes found of those tested inthe particulate fraction of the rat ventricles obtained from Dand DR rats in vivo, as identified by Western blot analysis andthe enhanced chemiluminescence technique (Figs. 6 and 7). ThePKC- $beta$ II and PKC- $gamma$ isozymes were present in low amounts in thesoluble fraction of the ventricles obtained from the D and DRrats but were absent from the particulate fraction of the ventriclesobtained from these groups of rats (Figs. 6 and 7). The contentof PKC- $alpha$ protein increased by 89.4 and 38.6% in the particulateand soluble fractions, respectively, of the hearts obtained fromthe BB/Wor D rats compared with the content of this PKC isozymein these fractions of hearts obtained from the BB/Wor DR rats(Fig. 7). Although the concentration of PKC- $delta$ protein was increasedby 24.2% in the particulate fraction of the hearts obtained fromthe D rats compared with that in the ventricles obtained fromthe DR rats, the amount of this PKC isozyme in the soluble fractionsof the ventricles obtained from these rats did not differ (Figs.6 and 7). The concentrations of both PKC- $beta$ II and PKC- $epsilon$ did notdiffer in the soluble and particulate fractions, respectively,of the ventricles obtained from the BB/Wor D and DR rats (Figs.6 and 7). Total PKC activity in the ventricles obtained from Drats was (mean ± SD) 985 ± 52 pg · mg protein¹ · min¹ (n = 4), whereas that of the DR rats was 768 ± 53 pg · mg protein¹ · min¹ (n = 4, P < 0.05). The PKC activity increased by 44.4 and 18.4%in the particulate and soluble fractions, respectively, obtainedfrom the ventricles of the BB/Wor D rats compared with the PKCactivity of the hearts obtained from the BB/Wor DR rats (Fig.8).

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Fig. 6. Typical Western blot of PKC- $alpha$ , PKC- $beta$ II, PKC- $gamma$ , PKC- $delta$ , and PKC- $epsilon$ in whole brain homogenate (B) used as a standard tissue containing multiple PKC isozymes and in soluble (cytosol) and particulate fractions (membrane) of heart ventricles obtained from BB/Wor rats with insulin-dependent diabetes mellitus (IDM; D) and BB/Wor rats without IDM (C). Molecular masses of isozymes (in kDa) are at left (for details, see METHODS AND MATERIALS).

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Fig. 7. Changes of isozyme content of PKC- $alpha$ , PKC- $beta$ , PKC- $delta$ , PKC- $gamma$ , and PKC- $epsilon$ in soluble (A) and membrane fractions (B) of ventricles of hearts obtained from BB/Wor diabetic (D) and diabetes-resistant (DR) rats. Each mean ± SD represents the responses from 5 animals/group. Data are expressed in gel density units. * Response significantly different from that of DR rats (P < 0.05).

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Fig. 8. Changes in the enzymatic activity of total PKC activity and PKC activity in cytosolic (soluble) and membrane (particulate) fractions of ventricles obtained from BB/Wor D and diabetes-resistant rats. Means ± SD represent responses from 4 rats/group. Data are expressed in pg phosphorylated substrate · mg protein¹ · min¹. * Response significantly different from that of DR rats (P < 0.05).

Gracilis muscle PKC isozyme content and PKC activity. PKC- $alpha$ and small amounts of PKC- $beta$ II were the predominant PKC isozymes in the soluble fraction of the freshly frozen gracilismuscle, whereas PKC- $alpha$ >> PKC- $delta$ >> PKC- $epsilon$ in the particulate fraction(Fig. 9). The gel density of both PKC isozymes increased in thegracilis muscle obtained from the D rat compared with the DR rat.However, PKC- $alpha$ increased by 438% (P < 0.05), whereas that of PKC- $delta$ increased by 92% (P < 0.05) (Fig. 10A). PKC activity in the particulatefraction of the gracilis muscle was greater than that of the ventricleand was increased in the gracilis muscle obtained from D ratscompared with that obtained from DR rats (Fig. 10A).

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Fig. 9. Typical Western immunoblot of isozyme content of PKC- $alpha$ , PKC- $beta$ , PKC- $gamma$ , PKC- $delta$ , and PKC- $epsilon$ in the brain (B) and soluble (cytosol) and particulate (membrane) fractions of the gracilis muscle obtained from BB/Wor DR rats (C) and BB/Wor D rats (D). Note presence of PKC- $alpha$ , PKC- $delta$ , and PKC- $epsilon$ in particulate fraction and the increase in PKC- $alpha$ and PKC- $delta$ in the gracilis muscle of the D rat compared with the control DR rat (for details see METHODS AND MATERIALS).

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Fig. 10. PKC activity (bars at left; nmol · mg protein¹ · min¹ for 20-min period) and PKC isozyme content (PKC- $alpha$ , PKC- $beta$ , PKC- $delta$ , or PKC- $epsilon$ ; gel density units/mm²) determined by Western immunoblot of freshly isolated and frozen gracilis muscle (A) and neutrophils (B) from BB/Wor diabetic rats and BB/Wor diabetes-resistant rats (control). Means ± SD represent responses from 5 animals/group. * Response significantly different from that of control rats (P < 0.05).

Neutrophil PKC isozyme content and PKC activity. The neutrophil content of the fractionated phagocytes was 99.9 ± 0.1% with 98 ± 0.4% viability based on exclusion of Evansblue dye. This was in agreement with previous findings (20).Small amounts of PKC- $alpha$ and PKC- $beta$ II and large amounts of PKC- $delta$ were the predominant PKC isozymes in the soluble fraction of thefreshly frozen neutrophils (data not shown), whereas PKC- $alpha$ andPKC- $delta$ were predominant in the particulate fraction of the freshlyisolated neutrophils. (Fig. 10B). The gel density of the PKC isozymesdid not increase in the soluble (data not shown) or particulate(Fig. 10B) fractions of the neutrophils obtained from the D ratscompared with the DR rats. However, basal neutrophil PKC activity,which was the highest when compared with that of the ventricleand gracilis muscle, increased by 23 ± 24% (P > 0.05) in the particulatefraction of the neutrophils obtained from D rats compared withthat obtained from DR rats (Fig. 10B).

	DISCUSSION

Top Abstract Introduction Materials Results Discussion References

This study demonstrates with the use of echocardiography, Doppler flowmetry, and hemodynamic measurements that during theearly incipient stages of IDM in the BB/Wor D rat interventricularseptal thickness, the E wave peak velocity of tricuspid inflow,and LV weight index were increased, and myocardial contractilityand the rate of relaxation were decreased compared with theseparameters in age-matched DR rats. Thus, in vivo, the early diabeticcardiomyopathy of the D rat is characterized by a less compliantLV and a restrictive right ventricle (RV) with increased septalthickness. Although we did not measure skeletal muscle functionin the D or DR rats, it is known that skeletal muscle dysfunctionoccurs during the progression of IDM, as well as enhanced susceptibilityto infections (4, 6, 19). The in vivo changes in cardiacfunction and structure reported herein were minimal and beforethe onset of fully expressed diabetic cardiomyopathy or impairedskeletal muscle function (33) were accompanied by selectiveincreases in particulate-bound PKC- $alpha$ and PKC- $delta$ isozymes, withundetectable changes in these or the PKC- $beta$ II or PKC- $epsilon$ isozymesin the soluble fraction. Moreover, they also occurred at a timewhen neutrophil PKC isozymes did not differ between the D andDR rats. This increase in PKC isozyme content was accompaniedby increases of the basal total, soluble, and particulate PKCactivity of the ventricles and the particulate fraction of thegracilis muscle, whereas that of the neutrophil did not changewhen obtained from the BB/Wor D rats compared with that of theBB/Wor DR rats. These findings lend support to the hypothesisthat sustained elevations of ventricular and gracilis muscle particulate(membrane) PKC activity and isozyme content occur before, andmay be responsible for, the early transition from normal to diseasedmyocardium and skeletal muscle during the development of diabeticmyopathies.

Cardiac function and structure. Most studies of diabetic cardiomyopathy in the BB/Wor diabetic rat model and humans have focused on LV abnormalities, themost consistent of which have been reduced LV compliance and diastolicdysfunction (4, 13, 14, 22, 26, 31, 38, 44).We are unaware of any reported echocardiographic studies in diabeticrats. However, echocardiographic evidence for abnormalities inLV function, diastolic function, and compliance in diabetic humanshas been demonstrated by several investigators (13, 22, 28,31). Interestingly, although both +LV dP/dt and $-$ LV dP/dt (relaxation)were depressed in the BB/Wor D rat compared with these parametersin the DR rat, the major functional and structural alterationin the BB/Wor D rat was detected in the interventricular septumand the RV when assessed by echocardiography and Doppler flowmetry.The increased E wave velocity present in the tricuspid inflowpattern as recorded by Doppler sonography may be indicative ofa restrictive pattern of ventricular filling (13, 22, 28,31). Although an increase in tricuspid E wave velocity may alsoreflect an increase in venous return (preload), it is unlikelythat cardiac output was increased in the BB/Wor diabetic ratsbecause similar increases of E wave velocity recorded from themitral valve were not forthcoming. Evidence for early RV involvementin experimental diabetic cardiomyopathy is also forthcoming fromthe histopathological evidence of more severe cardiomyopathy inthe RV compared with the LV in rats with STZ-induced diabetes(9, 38, 44). This is consistent with the experience ofmost investigators, who find that ~12 wk of hyperglycemia arenecessary to produce typical findings of LV dysfunction and overtdiabetic cardiomyopathy in BB/Wor D rats (4, 31). Thus theslight increase in interventricular septal thickness and the trendtoward increased LV mass associated with normal LV systolic pressure,reduced positive and negative LV dP/dt, and slightly impaireddiastolic function as determined in vivo by echocardiography andcardiac pressure measurements without in vitro functional changesin the isolated working heart are consistent with evidence thatthe BB/Wor D rats were studied at the incipient stages of diabeticcardiomyopathy in vivo.

PKC and diabetic cardiomyopathy. Elevated plasma levels of glucose have been shown to increase PKC activity in two major organ systems that are targets fordiabetes-mediated injury. These include the retinal capillaryendothelial cells in cell culture (33), cultured aortic smoothmuscle and endothelial cells (1, 15, 17, 35, 39, 40),and cardiac myocytes (2, 8, 16, 17, 25, 37). Diabetesalso increases the PKC content and activity in the hearts andvasculature of experimental animals and humans (1, 2, 8,15-17, 25, 36, 37, 41). Many factors have been suggestedto play a role in the transition from normal to diseased myocardiumin IDM. Among these are alterations in intracellular pH (40);derangements of intracellular metabolism of Ca²⁺, Ca²⁺ transport, and transmembrane permeability to Ca²⁺ (43, 44); changes in the isozyme patterns of myosin (13,43); impaired mitochondrial function (4, 6, 19, 44);altered utilization of glucose and fatty acids (6, 31, 41,43); decreased activity of cAMP (33); and increased activityof PKC (8, 16, 25, 26, 37, 42, 43). PKC may bethe most important of these diabetogenic factors because the obligatoryhyperglycemia of IDM can upregulate PKC (6, 16, 26, 41)and the PKC- $delta$ isozyme of PKC can modulate intracellular pH andalter intracellular and transmembrane Ca²⁺ metabolism in part by increasing Ca²⁺ influx through L-type Ca²⁺ channels (35) present in ventricular myocyte and skeletal musclemembranes (15, 21, 23, 29). Activation of cPKC- $delta$ and nPKC- $epsilon$ is also associated with myocardial ventricular hypertrophy, includingoverexpression of $beta$ -MHC, vMLC-2, ANF, and ACE (36, 39), andimpairment of myocardial contractility consequent to stimulationof $beta$ -MHC and vMLC-2 and phosphorylation of troponin and the troponin-tropomyosincomplex (15, 17, 21, 23, 24, 27, 36, 40). Thusmany of the changes in myocardial structure and cardiac and skeletalmuscle function in IDM may result from the combined activationand suppression of the actions of the PKC isozymes on variousbiochemical reactions of myocardial and skeletal muscle cellsand their surrounding supporting cells (18, 25, 27, 41).In support of this speculation are the findings that chronic administrationof a selective inhibitor of PKC- $beta$ to diabetic rats decreased thevascular and cardiac changes associated with STZ-induced diabetes(1, 17). Our finding of an increase in particulate but notsoluble PKC- $alpha$ and PKC- $delta$ protein in the ventricle and gracilismuscle, and increases in total, particulate, and soluble PKC activityin these same tissues when obtained in vivo from the BB/Wor Drat, whereas neutrophil PKC protein and activity did not differbetween the D and DR rat, is consistent with the reported increasesof DAG and particulate and soluble PKC activity in cardiac ventricularmyocytes obtained from STZ-induced diabetic and BB/Wor D ratscompared with that of control rats (8, 16, 25, 26, 37,42). Moreover, it suggests that these changes may be relatedto progression of the disease rather than to a genetic predispositionfor increased PKC in the BB/Wor D rat inasmuch as the neutrophilwas refractory to the changes. Also, the finding of overexpressionof PKC- $delta$ in the heart of the BB/Wor D rat may have clinical significancebecause PKC- $delta$ has been shown to modulate cardiac L-type Ca²⁺ channels expressed in Xenopus oocytes (34). Intracellular Ca²⁺ is increased and Ca²⁺ sequestration decreased in the myocardium of BB/Wor D rats, STZ-induceddiabetic animals, and humans with IDM and type II diabetes mellitus(2, 44). If the changes in PKC- $delta$ are found to precede theincrease of intraventricular and skeletal muscle Ca²⁺, then the changes in the PKC isozyme would be clearly importantrelative to the transition of normal myocardium and skeletal muscleto diabetes-induced cardiomyopathy and skeletal muscle myopathy.

The basal PKC activity of the whole heart increased in vivo early in the course of IDM when the changes in cardiac functionwere first manifest and overt cardiomyopathy was not yet evident.However, the change in total PKC activity was significantly smallerthan expected from the large changes in the content of PKC- $alpha$ andPKC- $delta$ . PKC- $epsilon$ has been suggested to be a major PKC isozyme in adultrat hearts (2) but did not increase in this study. We measuredfive isozymes of PKC. Because PKC represents a structurally homologousgroup of 12 isozymes that modulate the biochemical function ofproteins in a rapid and reversible manner (15, 21, 23, 36),it is possible, although speculative, that the mismatch betweentotal heart PKC activity and the increased PKC- $alpha$ and PKC- $delta$ proteinsreflected an increase of isozyme that was not fully active ora decrease in the activity or content of an isozyme that was notmeasured (15, 21, 23, 36). These postulates remain tobe resolved. However, it would not be inappropriate to suggestat this time that alterations in PKC isozyme patterns and activityare causal to the later cardiac and skeletal myopathies associatedwith IDM, because skeletal muscle function does not change thisearly in IDM (4, 6, 19). However, this model clearly supportsthe conclusion that the PKC isozyme patterns change and PKC activityis elevated in the ventricle and gracilis muscle of the BB/WorD rat in the early phase of the transition from normal to diseasedmuscle in IDM.

Another major finding of this study is that the isozyme profile of freshly isolated ventricles, neutrophils, and skeletalmuscle freshly obtained from BB/Wor D rats differed not only fromthat of the DR rat but also from that of myocytes incubated undercell culture conditions, a finding that has not been previouslyreported. Previous investigators have reported a preferentialincrease in PKC- $beta$ II isozyme in myocytes in cell culture obtainedfrom the diabetic rat myocardium and vasculature (1, 16,17, 36). This study not only failed to find particulate PKC- $beta$ IIisozyme in the ventricle, gracilis muscle, and neutrophil butfound the PKC- $beta$ isozyme was present in very low levels in thesoluble fraction and did not increase in the tissues obtainedfrom the BB/Wor D rat compared with those obtained from the BB/WorDR rat. Our inability to detect this isozyme in rat tissue wasnot due to technical reasons inasmuch as we were able to detectsignificant amounts of PKC- $beta$ II isozyme in freshly isolated ratbrains (Figs. 5 and 7). The length of the diabetes and the processof cell culture may explain these differences. First, our ratswere diabetic for 30-41 days, whereas the rats with STZ-induceddiabetes and the BB/Wor D and DR rats used in previous studieswere evaluated after 10-12 wk of diabetes (1, 16, 17, 29,36, 43). Thus the duration of the hyperglycemia characteristicof the diabetic state may have upregulated the PKC- $beta$ II isozyme(4, 23, 36, 43). Many cell lines and cells in cultureexhibit phenotypic and genotypic transformations that may limitthe extrapolation of data obtained to the intact cells from whichthey were derived in vivo. The peptide growth factors in cellculture medium and the cell culture process itself have been shownto revert many enzymes to their fetal phenotype (3, 5).Thus the predominant PKC isozyme of adult myocytes may be shiftedfrom that of PKC- $alpha$ , PKC- $delta$ , and PKC- $epsilon$ in vivo to that of the fetalPKC- $beta$ during cell culture (3, 5). Also, the specificityof inhibitors of PKC for an isozyme type must initially be performedin vitro using cultured cells or transformed cell lines (1,17) and the in vivo selectivity of these inhibitors on an isozymeis also usually inferred from the PKC isozyme(s) inhibited invitro. The selectivity and specificity of an inhibitor againsta PKC isozyme in vivo and in culture may differ. Thus the lengthof diabetes and the use of cell culture may have influenced thedifferent isozyme patterns observed herein and elsewhere (1,2, 17, 18, 21, 27, 30, 36). Finally, the differencein PKC isozymes reported herein and elsewhere (1, 2, 17,18, 21, 27, 30, 36) may result from our measurementof PKC isozymes as they occur in the basal state in contrast tothe phorbol ester-stimulated myocardial cells in culture. Eachtype of measurement is useful. However, the former reflects thePKC isozyme pattern in the intact tissue as it essentially occursin vivo under the conditions modulating the functionality of theheart. The latter reflects the response of the PKC system to theintroduction of a sudden and sustained stimulus to PKC.

Limitations of study. A major limitation of this study is that we measured whole ventricle PKC activity and we only measured five PKC isozymes,whereas previous studies measured the PKC activity and isozymeprofile of pure ventricular or atrial myocytes in cell culture(6, 16, 18, 21, 25, 42). We were able to detect increasesin several PKC isozymes as well as measure the PKC- $beta$ II isozymein the soluble fraction and PKC- $epsilon$ isozyme in the particulate fractionof the hearts and gracilis muscle obtained from both BB/Wor Dand DR rats. Thus it is unlikely that the small amount of proteinderived from the arteries and endothelium within the ventriclesor within the gracilis muscle could contribute significantly tothe PKC activity or mask the PKC isozyme profile of the largeramount of muscle. In support of this conclusion is the findingthat the relative density of the constitutive mRNA for PKC- $alpha$ ,PKC- $delta$ , PKC- $epsilon$ , and PKC- $zeta$ paralleled the relative density of thePKC isozyme proteins as determined by Western blot analyses.

A second limitation of this study, as stated above, is that the IDM produced changes in the content or the activity of thePKC isozymes that we did not measure. However, we measured themajor PKC isozymes known to be present in the myocytes. Additionalstudies are necessary to determine if IDM changes the content,distribution, or enzymatic activity of the remaining seven PKCisozymes.

A third limitation of this study is that it only measured the changes in PKC isozyme pattern and myocardial function and structureat one time point during the transformation from normal to diabeticcardiomyopathic heart. However, few studies have been conductedon the early myocardial changes associated with diabetes mellitus.The echocardiographic and interventricular septal measurementswere concordant in indicating that primary changes in the myocardiumof the BB/Wor diabetic rats were predominantly RV and septal inorigin and that these changes were consistent with the documentedeffects of PKC on cell growth (16, 21, 36). However, thisstudy does not reveal the precise meaning of the alteration inPKC isozyme pattern we observed. Although PKC- $alpha$ is ubiquitousin nature, specific functions have been assigned to some of themore esoteric of the PKC isozymes, such as alterations of L- andT-type Ca²⁺ channels by PKC- $delta$ and PKC- $epsilon$ , respectively (16, 21, 35).Speculatively, these PKC isozymes may represent a divergence incell transduction or lipid signaling and sustained cellular responsescontributing to the long-term structural changes of the myocardiumin IDM.

Conclusion. At an early stage during the development of diabetic cardiomyopathy (which is characterized by a restrictive RV, small decreasesof +LV dP/dt and $-$ LV dP/dt, and an increase in the interventricularseptal thickness and mass), total, particulate, and soluble PKCactivity of the whole heart is also increased. This is accompaniedby elevations in the particulate fraction of PKC- $alpha$ and PKC- $delta$ isozymes.Similar results were observed in gracilis muscle but not in thecirculating neutrophil. Because these isoforms of PKC can producechanges in intracellular pH, Ca²⁺, contractility, and cell growth characteristic of IDM, the datasupport the hypothesis that increased PKC activity and changesof the PKC isozyme profile may play an important role in the transitionfrom normal to abnormal myocardium and skeletal muscle in typeI diabetes mellitus.

	ACKNOWLEDGEMENTS

This research was supported by funds from the Department of Medicine, Section of Cardiology, Louisiana State University MedicalCenter, and by National Institute on Alcohol Abuse and AlcoholismGrants R01-AA-11224 and RO-1-AA-09816 (to S. S. Greenberg).

	FOOTNOTES

This manuscript was presented in part in abstract form on August 23, 1996, at the American Heart Association Conference onthe Normal, Hypertrophied, and Failing Myocardium (Snowbird, UT).

Address for reprint requests: T. D. Giles, Dept. of Medicine, Section of Cardiology, Louisiana State Univ. Medical Center, 1542 Tulane Ave., Rm. 334, New Orleans, LA 70112.

Received 22 May 1997; accepted in final form 13 August 1997.

	REFERENCES

Top Abstract Introduction Materials Results Discussion References

1. Birch, K. A., W. F. Heath, R. N. Hermeling, C. M. Johnston, L. Stramm, C. Dell, C. Smith, J. R. Williamson, and A. Reifel-Miller. LY290181, an inhibitor of diabetes-induced vascular dysfunction, blocks protein kinase C-stimulated transcriptional activation through inhibition of transcription factor binding to a phorbol response element. Diabetes 45: 642-650, 1996[Abstract].

2. Bogoyevitch, M. A., P. J. Parker, and P. H. Sugden. Characterization of protein kinase C isotype expression in adult rat heart. Protein kinase C-epsilon is a major isotype present, and it is activated by phorbol esters, epinephrine, and endothelin. Circ. Res. 72: 757-767, 1993[Abstract/Free Full Text].

3. Bourre, J. M., A. Faivre, O. Dumont, A. Nouvelot, C. Loudes, J. Puymirat, and A. Tixier-Vidal. Effect of polyunsaturated fatty acids on fetal mouse brain cells in culture in a chemically defined medium. J. Neurochem. 41: 1234-1242, 1983[Medline].

4. Carnaud, C. The contribution of animal models to the understanding of the pathogenesis of type 1 diabetes. Braz. J. Med. Biol. Res. 28: 925-929, 1995[Medline].

5. Conn, P. M. Cell Culture: Methods in Neuroscience 2 San Diego, CA: Academic, 1990.

6. Crisa, L., J. P. Mordes, and A. A. Rossini. Autoimmune diabetes mellitus in the BB rat. Diabetes Metab. Rev. 8: 4-37, 1992[Medline].

7. Dotta, F., and U. D. Mario. Antigenic determinants in type 1 diabetes mellitus. APMIS 104: 769-774, 1996[Medline].

8. Eckel, J., and H. Reinauer. Modulation of transmembrane potential of isolated cardiac myocytes by insulin and isoproterenol. Am. J. Physiol. 259 (Heart Circ. Physiol. 28): H554-H559, 1990[Abstract/Free Full Text].

9. Given, M. B., R. F. Lowe, C. R. Gelvin, G. E. Sander, and T. D. Giles. Preservation of left ventricular function and coronary flow by angiotensin I-converting enzyme inhibition in the hypertensive-diabetic Dahl rat. Am. J. Hypertens. 7: 919-925, 1994[Medline].

10. Greenberg, S. S., X. Zhao, J.-F. Wang, L. Hua, and J. Ouyang. cAMP and purinergic P_2y receptors upregulate and enhance inducible NO synthase mRNA and protein in vivo. Am. J. Physiol. 273 (Lung Cell. Mol. Physiol. 17): L967-L979, 1997[Abstract/Free Full Text].

11. Greenberg, S. S., J. Xie, X. Zhao, O. Jie, and T. D. Giles. An in vivo cytokine and endotoxin-independent pathway for induction of nitric oxide synthase II mRNA, enzyme, and nitrate/nitrite in alveolar macrophages. Biochem. Biophys. Res. Commun. 227: 160-167, 1996[Medline].

12. Gu, X., and S. P. Bishop. Increased protein kinase C and isozyme redistribution in pressure-overload cardiac hypertrophy in the rat. Circ. Res. 75: 926-931, 1994[Abstract/Free Full Text].

13. Hamby, R. I., S. Zoneraich, and L. Sherman. Diabetic cardiomyopathy. JAMA 229: 1749-1754, 1974[Abstract/Free Full Text].

14. Hiramatsu, K., N. Ohara, S. Shigematsu, T. Aizawa, F. Ishihara, A. Niwa, T. Yamada, M. Naka, A. Momose, and K. Yoshizawa. Left ventricular filling abnormalities in non-insulin-dependent diabetes mellitus and improvement by a short-term glycemic control. Am. J. Cardiol. 70: 1185-1189, 1992[Medline].

15. Hug, H., and T. F. Sarre. Protein kinase C isoenzymes: divergence in signal transduction? Biochem. J. 291: 329-343, 1993.

16. Inoguchi, T., R. Battan, E. Handler, J. R. Sportsman, W. Heath, and G. L. King. Preferential elevation of protein kinase C isoform beta II and diacylglycerol levels in the aorta and heart of diabetic rats: differential reversibility to glycemic control by islet cell transplantation. Proc. Natl. Acad. Sci. USA 89: 11059-11063, 1992[Abstract/Free Full Text].

17. Ishii, H., M. R. Jirousek, D. Koya, C. Takagi, P. Xia, A. Clermont, S. E. Bursell, T. S. Kern, L. M. Ballas, W. F. Heath, L. E. Stramm, E. P. Feener, and G. L. King. Amelioration of vascular dysfunctions in diabetic rats by an oral PKC beta inhibitor. Science 272: 728-731, 1996[Abstract].

18. Kariya, K., L. R. Karns, and P. C. Simpson. Expression of a constitutively activated mutant of the beta-isozyme of protein kinase C in cardiac myocytes stimulates the promoter of the beta-myosin heavy chain isogene. J. Biol. Chem. 266: 10023-10026, 1991[Abstract/Free Full Text].

19. Kastern, W., F. Lang, and I. Kryspin-Sorensen. The genetics of insulin-dependent diabetes in the BB rat. Curr. Top. Microbiol. Immunol. 156: 87-102, 1990[Medline].

20. Kolls, J., J. Xie, R. LeBlanc, T. Malinski, S. Nelson, W. Summer, and S. S. Greenberg. Rapid induction of messenger RNA for nitric oxide synthase II in rat neutrophils in vivo by endotoxin and its suppression by prednisolone. Proc. Soc. Exp. Biol. Med. 205: 220-229, 1994[Medline].

21. Liu, J. P. Protein kinase C and its substrates. Mol. Cell. Endocrinol. 116: 1-29, 1996[Medline].

22. Nishimura, R. A., P. R. Housmans, L. K. Hatle, and A. J. Tajik. Assessment of diastolic function of the heart: background and current applications of Doppler echocardiography. I. Physiologic and pathophysiologic features. Mayo Clin. Proc. 64: 71-81, 1989[Medline].

23. Nishizuka, Y. Protein kinase C and lipid signaling for sustained cellular responses. FASEB J. 9: 484-496, 1995[Abstract].

24. Noland, T. A., Jr., and J. F. Kuo. Protein kinase C phosphorylation of cardiac troponin T decreases Ca²⁺-dependent actomyosin MgATPase activity and troponin T binding to tropomyosin-F-actin complex. Biochem. J. 288: 123-129, 1992.

25. Okumura, K., N. Akiyama, H. Hashimoto, K. Ogawa, and T. Satake. Alteration of 1,2-diacylglycerol content in myocardium from diabetic rats. Diabetes 37: 1168-1172, 1988[Abstract].

26. Porte, D., Jr., and M. W. Schwartz. Diabetes complications: why is glucose potentially toxic? Science 272: 699-700, 1996[Medline].

27. Qu, Y., J. Torchia, T. D. Phan, and A. K. Sen. Purification and characterization of protein kinase C isozymes from rat heart. Mol. Cell. Biochem. 103: 171-180, 1991[Medline].

28. Riggs, T. W., and D. Transue. Doppler echocardiographic evaluation of left ventricular diastolic function in adolescents with diabetes mellitus. Am. J. Cardiol. 65: 899-902, 1990[Medline].

29. Rossini, A. A., J. P. Mordes, and A. A. Like. Immunology of insulin-dependent diabetes mellitus. Annu. Rev. Immunol. 3: 289-320, 1985[Medline].

30. Rybin, V., and S. F. Steinberg. Do adult rat ventriular myocytes express protein kinase C- $alpha$ ? Am. J. Physiol. 272 (Heart Circ. Physiol. 41): H2485-H2491, 1997[Abstract/Free Full Text].

31. Sampson, M. J., J. B. Chambers, D. C. Sprigings, and P. L. Drury. Abnormal diastolic function in patients with type 1 diabetes and early nephropathy. Br. Heart J. 64: 266-271, 1990[Abstract/Free Full Text].

32. Schaffer, S. W., S. Allo, S. Punna, and T. White. Defective response to cAMP-dependent protein kinase in non-insulin-dependent diabetic heart. Am. J. Physiol. 261 (Endocrinol. Metab. 24): E369-E376, 1991[Abstract/Free Full Text].

33. Schroeder, R. E., C. L. Doria-Medina, U. G. Das, W. I. Sivitz, and S. U. Devaskar. Effect of maternal diabetes upon fetal rat myocardial and skeletal muscle glucose transporters. Pediatr. Res. 41: 11-19, 1997[Medline].

34. Shiba, T., T. Inoguchi, J. R. Sportsman, W. F. Heath, S. Bursell, and G. L. King. Correlation of diacylglycerol level and protein kinase C activity in rat retina to retinal circulation. Am. J. Physiol. 265 (Endocrinol. Metab. 28): E783-E793, 1993[Abstract/Free Full Text].

35. Singer-Lahat, D., E. Gershon, I. Lotan, R. Hullin, M. Biel, V. Flockerzi, F. Hofmann, and N. Dascal. Modulation of cardiac Ca²⁺ channels in Xenopus oocytes by protein kinase C. FEBS Lett. 306: 113-118, 1992[Medline].

36. Steinberg, S. F., M. Goldberg, and V. O. Rybin. Protein kinase C isoform diversity in the heart. J. Mol. Cell. Cardiol. 27: 141-153, 1995[Medline].

37. Tanaka, Y., A. Kashiwagi, Y. Saeki, Y. Takagi, T. Asahina, R. Kikkawa, and Y. Shigeta. Effects of verapamil on the cardiac $alpha$ ₁-adrenoceptor signalling system in diabetic rats. Eur. J. Pharmacol. 244: 105-109, 1993[Medline].

38. Uusitupa, M. I., J. N. Mustonen, and K. E. Airaksinen. Diabetic heart muscle disease. Ann. Med. 22: 377-386, 1990[Medline].

39. Valentovic, M. A., C. W. Elliott, and J. G. Ball. The effect of streptozotocin-induced diabetes and insulin treatment on angiotensin converting enzyme activity. Res. Commun. Chem. Pathol. Pharmacol. 58: 27-39, 1987[Medline].

40. Venema, R. C., and J. F. Kuo. Protein kinase C-mediated phosphorylation of troponin I and C-protein in isolated myocardial cells is associated with inhibition of myofibrillar actomyosin MgATPase. J. Biol. Chem. 268: 2705-2711, 1993[Abstract/Free Full Text].

41. Williams, B., and R. L. Howard. Glucose-induced changes in Na⁺/H⁺ antiport activity and gene expression in cultured vascular smooth muscle cells. Role of protein kinase C. J. Clin. Invest. 93: 2623-2631, 1994.

42. Xia, P., T. Inoguchi, T. S. Kern, R. L. Engerman, P. J. Oates, and G. L. King. Characterization of the mechanism for the chronic activation of diacylglycerol-protein kinase C pathway in diabetes and hypergalactosemia. Diabetes 43: 1122-1129, 1994[Abstract].

43. Xiang, H., and J. H. McNeill. Protein kinase C activity is altered in diabetic rat hearts. Biochem. Biophys. Res. Commun. 187: 703-710, 1992[Medline].

44. Zarich, S. W., and R. W. Nesto. Diabetic cardiomyopathy. Am. Heart J. 118: 1000-1012, 1989[Medline].

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				S. W. Schaffer, C. B. Croft, and V. Solodushko Cardioprotective effect of chronic hyperglycemia: effect on hypoxia-induced apoptosis and necrosis Am J Physiol Heart Circ Physiol, June 1, 2000; 278(6): H1948 - H1954. [Abstract] [Full Text] [PDF]

				X. Liu, J. Wang, N. Takeda, L. Binaglia, V. Panagia, and N. S. Dhalla Changes in cardiac protein kinase C activities and isozymes in streptozotocin-induced diabetes Am J Physiol Endocrinol Metab, November 1, 1999; 277(5): E798 - E804. [Abstract] [Full Text] [PDF]

				S. Shigematsu, K. Yamauchi, K. Nakajima, S. Iijima, T. Aizawa, and K. Hashizume D-Glucose and insulin stimulate migration and tubular formation of human endothelial cells in vitro Am J Physiol Endocrinol Metab, September 1, 1999; 277(3): E433 - E438. [Abstract] [Full Text] [PDF]