Hindawi BioMed Research International Volume 2017, Article ID 1569235, 12 pages https://doi.org/10.1155/2017/1569235 Research Article Effects of Wenxin Keli on Cardiac Hypertrophy and Arrhythmia via Regulation of the Calcium/Calmodulin Dependent Kinase II Signaling Pathway XinyuYang,1,2YuChen,1,2,3YandaLi,1,2XiaomengRen,1,2 YanweiXing,1,2andHongcaiShang1,2 1TheKeyLaboratoryofChineseInternalMedicineoftheMinistryofEducation, DongzhimenHospitalAffiliatedtoBeijingUniversityofChineseMedicine,Beijing100700,China 2Guang’anmenHospital,ChineseAcademyofChineseMedicalSciences,Beijing100053,China 3FujianHealthCollege,Fuzhou350101,China CorrespondenceshouldbeaddressedtoYanweiXing;[email protected];[email protected] Received 28 November 2016; Accepted 5 February 2017; Published 9 May 2017 AcademicEditor:AlexanderN.Orekhov Copyright©2017XinyuYangetal.ThisisanopenaccessarticledistributedundertheCreativeCommonsAttributionLicense, whichpermitsunrestricteduse,distribution,andreproductioninanymedium,providedtheoriginalworkisproperlycited. WeinvestigatedtheeffectsofWenxinKeli(WXKL)ontheCalcium/CalmodulindependentkinaseII(CaMKII)signaltransduction pathwaywithtransverseaorticconstriction(TAC)rats.Echocardiographicmeasurementswereobtained3and9weeksafterthe surgery.Meanwhile,theactionpotentials(APDs)wererecordedusingthewhole-cellpatchclamptechnique,andwesternblotting wasusedtoassesscomponentsoftheCaMKIIsignaltransductionpathway.Atboth3and9weeksaftertreatment,thefractional shortening(FS%)increasedintheWXKLgroupcomparedwiththeTACgroup.TheAPD90oftheTACgroupwaslongerthanthat oftheShamgroupandwasmarkedlyshortenedbyWXKLtreatment.Westernblottingresultsshowedthattheproteinexpressions ofCaMKII,phospholamban(PLB),andryanodinereceptor2(RYR2)werenotstatisticallysignificantamongthedifferentgroupsat bothtreatmenttimepoints.However,WXKLtreatmentdecreasedtheproteinlevelandphosphorylationofCaMKII(Thr-286)and increasedtheproteinlevelandphosphorylationofPLB(Thr-17)andthephosphorylationofRYR2(Ser-2814).WXKLalsodecreased theaccumulationoftypeIIIcollagenfibers.Inconclusion,WXKLmayimprovecardiacfunctionandinhibitthearrhythmiaby regulatingtheCaMKIIsignaltransductionpathway. 1.Introduction in the cardiomyocyte size. A previous study in a cohort of 690 athletes has found that 36% of the athletes died as a Cardiovascular diseases are the most common threat to resultofcardiachypertrophy[4].Theseresultshighlightthe humanhealthworldwideandaretheleadingcauseofmor- importance of finding suitable agents for treating cardiac bidityamonghumans.Inmanycardiovasculardiseases,car- hypertrophy. diachypertrophyisacommonpathologicalprocess,andthe CaMK II belongs to the subfamily of multifunctional cardiacarrhythmiainducedbyitisthemostcommoncause Ser/Thrkinases,whichphosphorylateavarietyofsubstrates of sudden cardiovascular death. Cardiac hypertrophy is a andregulatenumerouscellularfunctions[5–8]thatareinti- maladaptive change in response to pressure overload and matelyinvolvedinheartdiseases[9–11].ActivationofCaMK is also an important risk factor for developing heart failure II is an important step in the signaling of cardiac hyper- [1]. Pathological hypertrophy is characterized by significant trophy.SeveralstudieshavedemonstratedthatCaMKIIplays changes in the size, shape, wall thickness, and contractile important functions in the development of cardiac hyper- functionofthecardiacchamber[2,3].Atthelevelofsingle trophybycausingimpairedgeneexpression[12].Increasing cardiomyocytes,hypertrophyissimplydefinedasanincrease understandingofCaMKIIanditseffectsontheheartlends 2 BioMedResearchInternational supporttoitspotentialasatherapeutictarget[13].Thecom- studyreceivedhumanecareincompliancewiththeNational pound KN93 (2-[N-(2-hydroxyethyl)]-N-(4-methoxyben- InstitutesofHealthGuidefortheCareandUseofLaboratory zenesulfonyl)amino-N-(4-chlorocinnamyl)-N-methylben- Animals. zylamine)hasbeenwidelyusedasapharmacologicaltoolto inhibitCaMKIIinseveralstudies[14–16]. 2.3.EstablishmentoftheTACModelandSham-OperatedRats. WenxinKeli(WXKL)isaChineseherbalextractdevel- The TAC surgery was performed in male Sprague-Dawley opedattheGuang’anmenHospitaloftheChineseAcademy rats as described previously [19, 20]. Briefly, the rats were ofChineseMedicalSciences,anditisthefirstChinesemed- anaesthetized by intraperitoneal injection of a 3% solution icinetobeapprovedbytheChinesestateforuseinarrhyth- of chloral hydrate (300mg/kg). The preparation process mia.ThemainingredientsofWXKLconsistofNardostachys included endotracheal intubation, positive pressure ventila- chinensisBatal,Codonopsis,notoginseng,amber,andRhizoma tion,andpreoperativerecordingbytwelve-leadECG.Then, Polygonati.Alargenumberofclinicaltrialshaveconfirmed thethoraxwasopened,anda4-0silksuturewaspassedunder that WXKL can increase coronary blood flow, decrease theaortabetweentheoriginsoftherightinnominateandthe myocardialoxygenconsumption,enhancemyocardialcom- leftcommoncarotidarteries.A6Gneedlewasplacedonthe pliance,improvemyocardialhypoxiatolerance,relieveante- ascending aorta, and the suture was snugly tied around the riorandposteriorcardiacloading,decreasemyocardialtissue needleandtheaorta.Theprobewasthenquicklyremoved. damageinpatientswithhighbloodpressure,anddecreasethe Theskinwasclosed,andtheratsweremaintainedonaheat- occurrence of arrhythmia [17]. This drug has been proven ingpaduntiltheyrecoveredfromtheanesthesia.TheSham- to be beneficial in the treatment of various diseases, such operated animals underwent an identical procedure but ascardiacarrhythmias,cardiacinflammation,cardiachyper- withouttheapplicationofligation.Aftersurgery,bothgroups trophy, and chronic heart failure [18]. In the present study, were given tap water and normal chow in different cages. wesoughttodeterminewhetherWXKLandKN93decrease Tocharacterizethemodel,echocardiographicmeasurements cardiachypertrophyandarrhythmiabyregulatingtheCaMK wereobtained3and9weeksafterthesurgeryusingaVivid IIsignaltransductionpathway. 7Dimensioncardiovascularultrasoundsystem(GEHealth- care,Fairfield,Connecticut,UnitedStates)asdescribedpre- 2.MaterialsandMethods viously[21].Theindexesfortheleftventricularposteriorwall thickness(LVPWS),leftventricularinternaldimensionsys- 2.1. WXKL. WXKL, consisting of Rhizoma Nardostachys, tole(LVIDs),andFS%wereshowninFigure2. notoginseng,Codonopsis,amber,andRhizomaPolygonati,was providedbytheBuChangGroup,Shandong,China.Accord- 2.4. Histological Examination. Rat heart samples were cut ingtothenationalpharmacopoeia(NationalPharmacopoeia into transverse sections and stained with hematoxylin and Committee, 2005), the total amount of Ginseng saponin eosin (H&E), Masson’s trichrome, and Sirius Red dye as Rg1 (C42H72O14), notoginseng saponin R1 (C47H80O18), and described previously [22]. The stained sections were exam- Ginseng saponin Rb1 (C54H92O23) should not be less than inedunderalightmicroscope(OLYMPUSBX51,Japan)and 17mg per bag (9g). The powdered WXKL compound was photographedat400xmagnificationformorphologicalanal- dissolvedindistilledwaterbeforeuse. ysis.Meanwhile,theratmyocardialcellswereprocessedfor transmissionelectronmicroscopy(H-600,Japan)according 2.2.AnimalGroupsandAdministrationofDrugs. Onehun- toroutineprocedures,aspreviouslydescribed[23]. dred male Sprague-Dawley rats (body weight: 140–160g), purchasedfromtheVitalRiverExperimentalAnimalCenter 2.5.IsolationofCardiacVentricularMyocytes. Singlecardiac (Beijing,China),wererandomlydividedintotwogroups:the ventricular myocytes were isolated from the hearts of the TACgroup(𝑛=75)andtheShamgroup(𝑛=25)byusinga rats as previously described [24] with slight modifications. random number table. The TAC rats underwent transverse Briefly,5minutesaftertheratswereheparinized(100U/mL aortic constriction surgery, and those in the Sham group 1mL/100gi.p.),theanimalswereanesthetizedwith3%chlo- underwentanidenticalprocedurebutwithouttheapplication ralhydrate(0.5mL/100gi.p.).Theheartswererapidlyexcised ofligation.The75TACratswererandomlyassignedtothree and mounted on the Langendorff apparatus and perfused 2+ treatment groups by using a random number table after viatheaortawithoxygenatedCa -freeTyrodesolutionfor ultrasoniccardiogramevaluation:theTACgroup(𝑛 = 25), 5 minutes and then with Ca2+-free Tyrode solution con- inwhichtheratsweretreatedwiththevehiclealone(distilled taining collagenase II (0.6mg/mL, Worthington, USA), water,1mL/kg/day)byoraladministration;theWXKLgroup trypsin (0.24mg/mL, Amresco, USA), and proteinase E (𝑛 = 25), in which the rats were treated with the WXKL (0.08mg/mL,Amresco,USA)for15–20minutesat37∘C.Sub- compound(4g/kg/day)byoraladministration;andtheKN93 sequently, the ventricular tissue was excised, cut into small group (𝑛 = 25), in which the rats were treated with KN93 piecesinadishcontainingKBsolution,andblowngentlyto (14𝜇mol/kg/day)byintraperitonealinjection.After3weeks obtainsingleventricularmyocytes.Thecellsweremaintained ∘ oftreatment,10ratswererandomlyselectedfromeachgroup at4 CintheKBsolutionuntiluse.Allthesolutionswerecon- ∘ for the experiment. After 9 weeks of treatment, there were tinuouslygassedwith95%O2and5%CO2at37 C.Thesingle 15 rats in the Sham group, 10 rats in the TAC group (5 rats ventricular myocytes selected for electrophysiological mea- died), 13 rats in the KN93 group (2 rats died), and 12 rats surementswererod-shaped,quiescent,andCa-tolerantand in the WXKL group (3 rats died). All animals used in this hadclearcross-striationswithasmoothandglossysurface. BioMedResearchInternational 3 2.6. Electrophysiological Recording. The whole-cell patch groupsweresignificantlylowerthanthoseoftheTACgroup clamptechniquewasusedtorecordtheAPsusinganAxo- (Figure1(e)).Overall,thevaluesforPW/BWat9weekswere patch700Bamplifier(AxonInstruments,USA)andthedata significantlyhigherthanthoseat3weeks. were analyzed with pCLAMP 9.2 software (Axon Instru- ments, USA). Borosilicate glass patch pipettes (resistance = 3.2.AssessmentofCardiacFunctionbyEchocardiography. We 3–5MΩ)werepulledusingaverticalpipettepuller(Narishige evaluatedcardiacfunctionbyacombinationofechocardio- pp-830, Japan). The cells were maintained in an external graphy measurements that included the LVPWS, FS%, and solutionfor5to10minutesafterperfusion,andthedatawere LVIDs(Figure2).Beforetreatment,comparedwiththeSham recordedafterpiercingthecellfor5minutestostabilizethe group, the LVPWS of the TAC, WXKL, and KN93 groups current.Datarecordingswereperformedatroomtempera- were significantly higher. After treatment for 3 weeks, the ∘ ture(22 C)within25minutestoavoidcurrentrundown.APs LVPWS of the KN93 and WXKL groups were not different wereinitiatedinthecurrentclampmodeatarateof1.0Hz from that of the TAC group. Interestingly, after treatment using30trainsofsuprathresholdcurrentpulses.Membrane for9weeks,theLVPWSbecamesignificantlythickerinthe capacitance was calculated using the manual whole-cell KN93 and WXKL groups compared with the TAC group capacitancecontrolsontheAxopatchamplifier. (Figure2(b)).Aftertreatmentfor3weeks,theFS%decreased in the TAC group compared with the Sham group, but it 2.7.WesternBlotAnalysis. Theanimalswereeuthanizedafter increasedintheWXKLgroupcomparedwiththeTACgroup. 3weeksand9weeksofdrugadministration,andtheirhearts After9weeks,theFS%intheKN93andWXKLgroupswas were immediately harvested and stored in liquid nitrogen significantlyhigherthanthatintheTACgroup(Figure2(c)). until western blot analyses were performed. The antibodies However, the LVIDs of the TAC group had no significant tothefollowingproteinswereused:CaMKIIdelta(1:1000, difference compared with those of the KN93 and WXKL AbcamCorporation.),phospho-CaMKII(1:1000,CellSig- groupsafter3weeksoftreatment,buttheLVIDsdecreasedin naling Technology Inc.), PLB (G-18) (1:200, Santa Cruz theKN93andWXKLgroupscomparedwiththeTACgroup BiotechnologyInc.),p-phospholamban-R(1:200,SantaCruz aftertreatmentafter9weeksoftreatment(Figure2(d)). BiotechnologyInc.),andryanodinereceptor2(1:1000,Milli- poreCorporation.).Theproteinswereseparatedby10%SDS- 3.3.EffectsofWXKLandKN93onMyocardialCellMorphol- PAGEandtransferredontonitrocellulosemembranes,which ogyinaRatModelofCardiacHypertrophyInducedbyTAC. werethenincubatedwithantibodiesat4∘C.Themembranes After 9 weeks of treatment, we isolated single ventricular werefurtherincubatedfor2hoursatroomtemperature.ECL myocytes through enzymatic hydrolysis. After allowing the visualizationwasperformed,andaGeneGnomeGelImaging cells to adhere to slides, the cells with neat edges and clear System (Syngene Co.) was used to capture the resulting stripes were observed under a microscope. Compared with images.ImageJ(Image-Proplusanalysissoftware)wasused thoseintheShamgroup,thesingleventricularmyocytesin toanalyzethegelimages. the TAC group were larger (Figure 3). In addition, in the KN93andWXKLgroups,thecellmorphologywasimproved, and the degree of myocardial hypertrophy was decreased 2.8.StatisticalAnalyses. Allexperimentaldatawereexpressed asthemeans±SD.Thedatawerestatisticallyevaluatedusing comparedwiththatintheTACgroup. one-wayanalysisofvariance(ANOVA),andaposthocanaly- 3.4.ChangesintheMicrostructureoftheMyocardialTissuein sis was performed using Fisher’s least significant difference aRatModelofCardiacHypertrophyInducedbyTAC. Stained (LSD)test.TheSPSSprogram(version20.0)wasusedforthe analyses. A probability of 𝑃 < 0.05 was considered statis- sectionswereobservedunderalightmicroscope,andphotos were taken under 400x magnification. Collagen deposition ticallysignificant.ThepCLAMP9.2software(AxonInstru- wasobservedunderordinarylightmicroscope.Theresultsof ments, USA) and Origin 6.1 software (MicroCal Software, Masson’strichromestainingshowedthatthecollagenfibers USA)wereusedforthedataacquisitionandanalysis. were stained green. The cytoplasm and muscle fibers were stainedred.Theredbloodcellswerestainedorange,andthe 3.Results nuclei were stained blue-brown (Figure 4(a)). In the Sirius Red staining, the collagen fibers were stained red, and the 3.1. Effects of Treatment with WXKL and KN93 for 3 and nucleiwerestainedblue(Figure4(b)). 9 Weeks on Cardiac Morphology. The extent of myocardial Aftertreatmentfor3weeks,Masson’strichromestaining fibrosiswasimprovedintheKN93andWXKLgroupscom- showedthattheTACgrouphadfibrosis,andcollagendepo- paredwiththeTACgroupafter3and9weeksoftreatment sitionwasapparent.Inaddition,aftertreatmentfor9weeks, (Figure 1(c), HE staining 400x magnification). At 3 and 9 collagen deposition in the TAC group was even more pro- weeks,theratiosofheartweighttobodyweight(HW/BW) nounced, and the degree of heart failure was significantly of the TAC group were significantly higher than those of increased. In contrast, in the KN93 and WXKL groups, the the Sham group, but those of the KN93 and WXKL groups extent of collagen deposition was greatly decreased (Fig- werelessthanthevaluesfromtheTACgroup(Figure1(d)). ure4(a)).Asviewedunderalightmicroscope,theredstain- Meanwhile, the ratios of pulmonary weight to body weight ingshowedthatthedegreeoffibrosiswasthemostintensein (PW/BW)ofTACgroupwereonlyslightlyhigherthanthose the TAC group. However, fibrosis in the WXKL group was oftheShamgroup,buttheratiosfromtheKN93andWXKL significantly decreased at 9 weeks (Figure 4(b)). Under a 4 BioMedResearchInternational 3 weeks 9 weeks Sham TAC KN93 WXKL Sham TAC KN93 WXKL (a) (b) (c) TAC TAC 5 8 ∗ 󳵳󳵳 󳵳󳵳 󳵳󳵳 mg/g) 34 󳵳# 󳵳# 󳵳# 󳵳# mg/g) 6 󳵳 󳵳# 󳵳# 󳵳# 󳵳# ( ( 4 W W 2 B B W/ W/ 2 1 H P 0 0 Sham TAC93KN WXKL Sham TAC93KN WXKL Sham TAC93KN WXKL Sham TAC93KN WXKL 3 weeks 9 weeks 3 weeks 9 weeks 3 weeks 3 weeks 9 weeks 9 weeks (d) (e) Figure1:(a)RepresentativeimagesofheartsfromtheSham(𝑛=5),TAC(𝑛=5),KN93(𝑛=5),andWXKL(𝑛=5)groupsat3and9weeks aftertreatment.Scale:1cm.(b)Representativeimagesofthelargestcross-sectionoftheheartfromeachgroupat3and9weeks(𝑛=5).(c) Representativeimagesofleftventricularapicalbiopsyofeachgroupat3and9weeks(H&Estainingat400xmagnification;𝑛=5).(d)Ratios ofheartweighttobodyweight(HW/BW)areshown(𝑛=5).(e)Ratiosofpulmonaryweighttobodyweight(PW/BW)areshownat3and 9weeks.(𝑛 = 5).󳵳𝑃 < 0.05and󳵳󳵳𝑃 < 0.01versustheShamgroup.#𝑃 < 0.05versustheTACgroup.∗𝑃 < 0.05versustheTACgroupat3 weeks. polarizedlightmicroscope,SiriusRedstainedthetypeIcol- ridgeswerestillbroken.Aftertreatmentfor9weeks,inthe lageninredoryellowandthetypeIIIcollageningreen.Sirius Sham group, the myocardial cells were basically complete, Red-stainedsectionsclearlydisplayedthetypeIandtypeIII andthearrangementofthefilamentswasmoreregular.The collagen fibers (Figure 4(c)). The results showed that the structureofthemitochondriawasalsonormal.Onceagain,in typeIcollagenfiberswerearrangedclosely,showingstrong theTACgroup,themyocardialcellsweredissolvedtoamuch refraction, and they appeared bright orange red or bright greaterextent,andtheirarrangementwasmoredisordered. yellow.Incontrast,thestainingfortypeIIIcollagenfiberswas Themorphologyofthemitochondriawasalsosubstantially veryweakandnotasapparent. altered, and the crest had been fractured. However, after KN93 and WXKL drug treatment, the myocardial cells 3.5. Ultrastructural Changes in Cardiac Myocytes in a Rat showedslightrecovery,buttherewasstillasignificantchange ModelofCardiacHypertrophyInducedbyTAC. Aftertreat- inthemorphologyofmitochondria(Figure5). ment for 3 weeks, analysis of the ultrastructure of cardiac myocytes showed that the myocardial cells of the Sham 3.6. Effects of WXKL and KN93 on the APs after Treatment group were arranged in a compact manner, and the muscle for3and9Weeks. TheAPswererecordedbyapplicationofa sections were clear and complete. The mitochondrialstruc- 900-pAcurrentpulsewithadurationof3msat1Hzinthe turewasnormal,andtherewereabundantglycogengranules. currentclampmode.Aftertreatmentfor3weeks,theAPD90 However,intheTACgroup,manyofthecardiacmusclecells wasslightlyprolongedintheTACgroupcomparedwiththat hadbeendissolved,andsomegapsappeared.Themitochon- in the Sham group (Figure 6(a)). The APD90 values of the dria were swollen, and the ridges were broken. After KN93 ShamandTACgroupswere139.0±9.3msand150.3±11.6ms, andWXKLdrugtreatment,somemyocardialcellshadbeen respectively (Figure 6(c)). After treatment with KN93 and dissolved, the mitochondria still appeared swollen, and the WXKL, the APD90 changed slightly to 146.4 ± 6.5ms and BioMedResearchInternational 5 Vehicle Vehicle KN93 WXKL m 3 weeks c 1 m 9 weeks c 1 Sham TAC (a) 0.45 ∗󳵳 # 󳵳 # 70 󳵳 LVPWS (cm) 000...334050 ∗󳵳󳵳󳵳 󳵳󳵳# ∗## FS (%) 60 󳵳 # 󳵳#∗# 󳵳∗ 0.25 50 0 3 9 0 3 9 Weeks Weeks Sham KN93 Sham KN93 TAC WXKL TAC WXKL (b) (c) 0.7 󳵳∗ m) S(c 0.6 󳵳󳵳##∗∗ VID #∗ L 0.5 0 3 9 Weeks Sham KN93 TAC WXKL (d) Figure2:(a)TypicalechocardiographyimagesfromtheSham(𝑛=10),TAC(𝑛=10),KN93(𝑛=10),andWXKL(𝑛=10)groupsat3and 9weeks.Scale:0.5cm.(b)LVPWSofeachgroup(𝑛 = 10).(c)FS%ofeachgroup(𝑛 = 10).(d)LVIDsofeachgroup(𝑛 = 10).󳵳𝑃 < 0.05 versustheShamgroup.#𝑃<0.05versustheTACgroup.∗𝑃<0.05versuscorrespondingvaluesat3weeks. 143.4 ± 4.1ms, respectively. The WXKL group thus showed 3.7. Effects of WXKL and KN93 on the Expression of CaMK ashortenedAPD90.Aftertreatmentfor9weeks,theAPD90 II and Related Proteins. Western blotting analysis was per- wassignificantlyprolongedintheTACgroupcomparedwith formedtoexaminetheexpressionofCaMKII,Thr-286,PLB, theShamgroup(Figure6(b)).APD90 oftheShamandTAC Thr-17,RYR2,andSer-2814intheleftventricularapexamong groupswere142.7±3.9msand175.4±4.2s,respectively(Fig- thefourexperimentalgroups(Figure7(a)). ure6(c)).AftertreatmentwithKN93andWXKL,theAPD90 Aftertreatmentfor3andfor9weeks,thedifferenceinthe changed significantly to 160.4 ± 5.0ms, and 150.5 ± 4.6ms. expressionofCaMKIIwasnotstatisticallysignificantamong TheresultsthusshowedthatWXKLandKN93shortenedthe anyofthegroups(Figure7(b)).However,thelevelofThr-286 APD90. was increased in the TAC group compared with that in the 6 BioMedResearchInternational Sham TAC (a) (b) TAC + KN93 TAC + WXKL (c) (d) Figure3:SingleventricularmyocytesfromtheSham(a),TAC(b),KN93(c),andWXKL(d)group(400x). Shamgroup.ThelevelsofThr-286intheWXKLandKN93 remodeling and tissue remodeling in hypertrophic cardiac groupsweresignificantlydecreasedcomparedtointheTAC myocytes. group(Figure7(c)).Therewasasimilartrendinthechange Cardiac hypertrophy is a common pathological change aftertreatmentbothfor3weeksandfor9weeksonthelevels thatincreasestheincidenceandmortalityinmanycardiovas- ofThr-286. culardiseases.Thesechangesarefrequentlyinducedbyelec- The protein expression of PLB was not statistically sig- tricalremodelingandgenesisofarrhythmia.Theresultsfrom nificant after treatment for 9 weeks (Figure 7(d)). At both histology and immunohistochemistry analyses showed that treatmenttimepoints,theproteinexpressionofThr-17was WXKLandKN93hadasignificanteffectonthehypertrophic significantlydecreasedintheTACgroupcomparedwiththe myocardium.H&EandMasson’strichromestainingshowed Shamgroup.However,thelevelsofThr-17intheWXKLand thatthecardiomyocytesintheTACgroupweresignificantly KN93groupswereincreasedaftertreatment(Figure7(e)). larger and more loosely arranged. Cardiac fibrosis is a At both 3 and 9 weeks after treatment, the difference commonresponseofthehearttomanyformsofinjuryand in the level of RyR2 protein expression was not statistically isthekeypathologicalprocessinvariouscardiovasculardis- significantamongthedifferentgroups(Figure7(f)).Atboth eases [25]. In cardiac fibrosis, excessive collagen deposition treatment time points, however, the levels of Ser-2814 were and extracellular matrix accumulation result in myocardial decreasedintheTACgroupcomparedwiththeShamgroup, hypertrophy,cardiacdysfunction,andarrhythmias[26–28]. whereasitwashigherthanintheTACgroupintheWXKL Theexperimentalresultsrevealedthat,intheTACgroup,the andKN93groups(Figure7(g)). gap between cells had widened and the residual number of myocardialcellsdecreased,showingoverallfibrosis.Micro- 4.Discussion graphsindicatedthatWXKLandKN93improvedthetissue morphology.Theenhancementofcollagendepositionplays This study revealed that WXKL and KN93 significantly animportantroleinadverseremodelingofthecardiactissue decreasedthedevelopmentofcardiachypertrophy,thussug- [29]. Hence, stained sections were observed under a light gestingthatWXKLandKN93preservecardiacfunctionafter microscope, and the results showed that KN93 and WXKL TACinrats.Ourresultsalsoshowedthatthebeneficialeffects greatlydecreasedthedegreeofcollagendeposition.Theultra- of WXKL and KN93 might be attributed to the shortening structure of cardiac myocytes showed that the myocardial of APD90 and regulation of the CaMK II signal transduc- cells in rats also showed slight recovery after KN93 and tion pathway, thus eventually improving cardiac electrical WXKL drug treatments. Thus, WXKL and KN93 improved BioMedResearchInternational 7 Vehicle Vehicle KN93 WXKL 3 weeks 9 weeks Sham TAC (a) Vehicle Vehicle KN93 WXKL 3 weeks 200𝜇M 9 weeks Sham TAC (b) Vehicle Vehicle KN93 WXKL 3 weeks 9 weeks Sham TAC (c) Figure4:Representativeimagesof(a)Masson’strichromestainingmethodtoevaluatecardiacfibrosisofeachgroupat3and9weeks(𝑛=5), (b)SiriusRedstainingtoevaluatecardiacfibrosisofeachgroupat3and9weeks(𝑛=5),and(c)SiriusRedstainingtoevaluatecardiacfibrosis ofeachgroupat3and9weeksunderpolarizedlight(𝑛=5). 8 BioMedResearchInternational Sham TAC KN93 WXKL 3 weeks 9 weeks Sham TAC Figure5:Theultrastructureofmyocardialcellsineachgroupat3and9weeks(𝑛=5)(Magnification10,000x). cardiac fibrosis and decreased the degree of cardiac hyper- that WXKL and KN93 contributed to the improvement of trophy. cardiacfunctionandinhibitedtheprocessofcardiachyper- Cardiacfibrosiscannotonlycausecardiachypertrophy trophy. but also affect cardiac function. It can also cause substitu- Proper functioning of the heart depends on normal tion of the myocardium with nonfunctional fibrotic tissue, actionpotential,whichinturndependsonthenormalfunc- thus leading to impaired ventricular systolic and diastolic tioningofionchannels.Theabnormalitythatismostcom- functions, as well as atrial and ventricular arrhythmias and monlyfoundinanimalmodelsofcardiachypertrophyisthe heart failure [30, 31]. Here, we evaluated cardiac function prolongation of the APD [33–35]. It has been shown that through a combination of echocardiography measurements CaMK II inhibition has little effect on APD in a transgenic thatincludedtheparametersLVPWS,FS%,andLVIDs.After mouse with increased endogenous CaMK II activity [36]. treatmentfor3weeks,theLVPWSoftheKN93andWXKL However,treatmentwithKN93hasbeenshowntocontribute groups were not any thinner than that in the TAC group. totheshorteningofAPD[37].Inourmodel,wefoundthat Interestingly,aftertreatmentfor9weeks,theLVPWSwassig- theAPDoftheTACgroupwassignificantlyprolongedcom- nificantlythickerintheKN93andWXKLgroupscompared paredtothatoftheShamgroupafter3weeks,aresultcon- with the TAC group. These results showed that myocardial sistentwithresultsfrompreviousstudies[38,39].Aftertreat- hypertrophyhadformedafter3weeks,andWXKLandKN93 mentwithKN93andWXKL,theAPD90changedslightly,but hadaneffectofdecreasinghypertrophy.However,thecardiac thischangewasnotstatisticallysignificant.After9weeksof chamberswereenlarged,andthemyocardiumbecamethin- treatment,theresultsshowedthatWXKLandKN93further nerintheTACgroupafter9weeks.Afterboth3and9weeks shortenedtheAPD90.Becausesomestudieshavereportedthe oftreatment,theratiosofHW/BWandPW/BWoftheTAC useofWXKLforthetreatmentofpatientswitharrhythmia, group were higher than those of the Sham group, but the testing this parameter may be a reasonable and effective ratiosoftheKN93andWXKLgroupswerelessthanthatof choice[39,40].Thus,thispaperinvestigatedtheantiarrhyth- theTACgroup.Theenlargementoftheventricleandincrease mic effects of WXKL and KN93 in the TAC model using incardiacweightresultinadecreaseincardiacfunction,thus an electrophysiological technology. Other studies have also resulting in cardiac decompensation [32]. After 3 weeks of demonstrated that increased CaMK II activity is linked not treatment, the FS% decreased in the TAC group compared only to cardiomyopathy [41] but also to fatal arrhythmias, with the Sham group, but it increased in the WXKL group owing to the prolongation of APDs and development of compared with the TAC group. After 9 weeks of treatment, prematuredepolarization. the FS% of the KN93 and WXKL groups was significantly CaMKIIoverexpressioncontributestothedevelopment higherthanthatoftheTACgroup.However,theLVIDsofthe ofheartfailure[42],isassociatedwitharrhythmias[43–46], TAC group were significantly different from those of the and has detrimental consequences in irreversible ischemia KN93 and WXKL groups after 3 weeks, but, after 9 weeks and perfusion injury [47]. CaMK II is one of the most 2+ oftreatment,theLVIDsdecreasedintheKN93andWXKL important regulators of intracellular Ca -cycling and acts groupscomparedwiththeTACgroup.Theseresultsshowed through phosphorylation of various proteins such as RyR2 BioMedResearchInternational 9 20mV 50ms 3ms 900pA Sham Sham TAC TAC KN93 KN93 WXKL WXKL −75mV 1HZ −75mV 1HZ 3 weeks 9 weeks (a) (b) 200 󳵳 ∗∗ # ∗∗ ## 150 ms) ( D90 100 P A 50 0 m C 3 L m C 3 L Sha TA KN9 WXK Sha TA KN9 WXK 3 weeks 9 weeks 3 weeks 9 weeks (c) Figure6:RepresentativeAPtracesrecordedfromeachgroup.(a)APsofeachgrouptreatedfor3weeks(𝑛=5).(b)APsofeachgrouptreated for9weeks(𝑛=5).(c)APD90ofeachgroupaftertreatmentwithKN93and5g/LWXKLfor3weeksand9weeks(𝑛=5).∗∗𝑃<0.01versus theShamgroup.#𝑃<0.05and##𝑃<0.01versustheTACgroup.󳵳𝑃<0.05versustheTACgroupafter3weeks. andPLB[48].WhenCaMKIIexpressionandactivationare Nevertheless, WXKL and KN93 also significantly increased 2+ increased, RyR2 phosphorylation and the diastolic SR Ca theexpressionofSer-2814.Thesepossiblyenhancetheability 2+ leakagearealsoincreased[49];thisdiastolicSRCa leakcan tomodulatetheCaMKIIsignaltransductionpathway.This initiateDADsinwhichthedepolarizingcurrentconsistsofan maybethemostimportantmechanismbywhichWXKLand inwardNa+/Ca2+exchange[50].However,dephosphorylated KN93inhibitcardiachypertrophy. PLBinhibitsSERCA2aactivity,whereasthephosphorylation of PLB by cAMP-dependent protein kinase or CaMK II 5.Conclusions 2+ reverses SERCA2a inhibition, thus increasing Ca uptake into the luminal SR [51]. In the present study, the protein Insummary,thepresentstudyevaluatedtheeffectsofWXKL expressionofThr-286wassignificantlyincreasedintheTAC and KN93 on the expression of CaMK II and on the elec- group.WXKLandKN93significantlydecreasedthelevelof trophysiologicalparametersinTACrats.Theresultsdemon- Thr-286inratswithTAC.WXKLandKN93alsoincreased stratedthattheprolongationofAPD90resultingfromcardiac the level of Thr-17 in rats with cardiac hypertrophy. The hypertrophy was the electrophysiological mechanism caus- protein levels of RyR2 slightly recovered after WXKL and ing cardiac arrhythmias, and KN93 and WXKL shortened KN93 treatment, but there were no significant differences. the process and improved electrical remodeling. We also 10 BioMedResearchInternational 3 weeks 9 weeks VehicleVehicleKN93WXKLVehicleVehicleKN93WXKL CaMKII 50 p-CaMKII 50 PLB 47 p-PLB 27 Da) k ( RYR2 233 p-RYR2 233 GAPDH 37 Sham TAC Sham TAC (a) ADPH (Folds) 0011....6802 ∗ ADPH (Folds) 0011....6802 ∗∗ # # ∗∗ # # DPH (Folds) 0011....6802 ∗ MKII/G 00..24 MKII/G 00..24 LB/GA 00..24 Ca 0.0 Ca 0.0 P 0.0 Sham TAC KN93 WXKL Sham TAC KN93 WXKL p- Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL 3 weeks 9 weeks 3 weeks 9 weeks 3 weeks 9 weeks 3 weeks 3 weeks 9 weeks 3 weeks 9 weeks 9 weeks (b) (c) (d) DPH (Folds) 0011....6802 ∗∗ ## ## ∗∗ ## ## ADPH (Folds) 0011....6802 ADPH (Folds) 0011....6802 ∗ # ## ∗∗ ## ## LB/GA 00..24 YR2/G 00..24 YR2/G 00..24 p-P 0.0 R 0.0 p-R 0.0 Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL Sham TAC KN93 WXKL 3 weeks 9 weeks 3 weeks 9 weeks 3 weeks 9 weeks 3 weeks 3 weeks 3 weeks 9 weeks 9 weeks 9 weeks (e) (f) (g) Figure7:(a)TheexpressionofCaMKIIandrelatedproteinsintheCaMKIIsignaltransductionpathwayintheleftventricularareasafter treatmentfor3and9weekswereanalyzedbywesternblotting.(b)TheexpressionofCaMKII(𝑛 = 5).(c)Theexpressionofp-CaMKII (Thr-286)(𝑛=5).(d)TheexpressionofPLB(𝑛=5).(e)Theexpressionofp-PLB(Thr-17)(𝑛=5).(f)TheexpressionofRyR2(𝑛=5).(g) Theexpressionofp-RyR2(Ser-2814)(𝑛 = 5).∗𝑃 < 0.05and∗∗𝑃 < 0.01versustheShamgroup.#𝑃 < 0.05and##𝑃 < 0.01versustheTAC group.