RESEARCHARTICLE The effect of Bacopa monnieri on gene expression levels in SH-SY5Y human neuroblastoma cells How-WingLeung1☯,GabrielFoo1‡,GokulakrishnaBanumurthy1‡,XiaoranChai1‡, SujoyGhosh1‡,ToraMitra-Ganguli2¤*,AntoniusM.J.VanDongen1☯ 1 PrograminNeuroscienceandBehavioralDisorders,Duke-NUSMedicalSchool,Singapore,Singapore, 2 GlaxoSmithKlineConsumerHealthcare,Gurgaon,Haryana,India a1111111111 ☯Theseauthorscontributedequallytothiswork. a1111111111 ¤ Currentaddress:IndianInstituteofTechnologyTirupati,AndhraPradesh,India a1111111111 ‡Theseauthorsalsocontributedequallytothiswork. a1111111111 *[email protected] a1111111111 Abstract BacopamonnieriisaplantusedasanootropicinAyurveda,a5000-year-oldsystemoftradi- OPENACCESS tionalIndianmedicine.Althoughbothanimalandclinicalstudiessupporteditsroleasa Citation:LeungH-W,FooG,BanumurthyG,Chai memoryenhancer,themolecularandcellularmechanismunderlyingBacopa’snootropic X,GhoshS,Mitra-GanguliT,etal.(2017)The actionarenotunderstood.Inthisstudy,weuseddeepsequencing(RNA-Seq)toidentifythe effectofBacopamonnieriongeneexpression levelsinSH-SY5Yhumanneuroblastomacells. transcriptomechangesuponBacopatreatmentonSH-SY5Yhumanneuroblastomacells. PLoSONE12(8):e0182984.https://doi.org/ WeidentifiedseveralgeneswhoseexpressionlevelswereregulatedbyBacopa.Biostatisti- 10.1371/journal.pone.0182984 calanalysisoftheRNA-Seqdataidentifiedbiologicalpathwaysandmolecularfunctionsthat Editor:NatarajanAravindan,Universityof wereregulatedbyBacopa,includingregulationofmRNAtranslationandtransmembrane OklahomaHealthSciencesCenter,UNITED transport,responsestooxidativestressandproteinmisfolding.Pathwayanalysisusingthe STATES IngenuityplatformsuggestedthatBacopamayprotectagainstbraindamageandimprove Received:February24,2017 braindevelopment.Thesenewlyidentifiedmolecularandcellulardeterminantsmaycontrib- Accepted:July27,2017 utetothenootropicactionofBacopaandopenupanewdirectionofinvestigationintoits Published:August23,2017 mechanismofaction. Copyright:©2017Leungetal.Thisisanopen accessarticledistributedunderthetermsofthe CreativeCommonsAttributionLicense,which permitsunrestricteduse,distribution,and reproductioninanymedium,providedtheoriginal authorandsourcearecredited. Introduction DataAvailabilityStatement:Allrelevantdataare Bacopamonnieri(Bacopa),alsoknownasBacopamonniera,Herpestismonniera,waterhyssop withinthepaper. orBrahmi,haslongbeenusedinIndiantraditionalmedicine(Ayurveda)asabraintonicto Funding:Theworkwassupportedbyagrantfrom enhancememoryperformance,learningandconcentration[1,2].Thesetraditionalclaims GlaxoSmithKlinetoAV,whichwereinvolvedinthe haverecentlybeensupportedbyseveralanimalandclinicalstudies.Animalstreatedchroni- studydesign.Thefundershadnoroleindata callywithBacopashowedbetteracquisitionandimprovedretentioninlearningtasks[3–11]. collectionandanalysis,decisiontopublish,or Similarly,clinicalstudiesandameta-analysisofrandomizedcontroltrialsalsodemonstrated preparationofthemanuscript.Thefunderprovided thatchronicoraladministrationofBacopa(overaperiodofmorethan12weeks)tohealthy supportintheformofsalariesforauthorsHL,GF subjectsresultedinimprovementsinthesubjects’informationprocessingspeed,freerecall, andGB,butdidnothaveanyadditionalroleinthe studydesign,datacollectionandanalysis,decision verbalmemoryandlearning.Bacopatreatmentalsoresultedinadecreaseinanxiety,which PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 1/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells topublish,orpreparationofthemanuscript.The improvedlearning[12–19].Withitslowtoxicityrisksandapparentbeneficialeffectsasanoot- specificrolesoftheseauthorsarearticulatedinthe ropic[20–22],Bacopahasbeenextractedandmarketedasadietarysupplement(KeenMindor ‘authorcontributions’section. CDRI08,SohoFlordisInternational)anditsproductionandimportsaretightlyinspectedby Competinginterests:Thisworkissupportedbya theFoodandDrugAdministration(FDA)(https://tinyurl.com/ybkmhfes).Notwithstanding grantfromGlaxoSmithKlinetoAV.Thefunder itswideavailability,themechanismsofactionofBacopahaveyettobedelineated.Several providedsupportintheformofsalariesas mechanismshavebeenproposedconcerningthenootropiceffectsofBacopa.Theseincluded indicatedintheFundingStatement.This alterationofthelevelsofseveralneurotransmitters,includingserotonin(5-hydroxytrypta- commercialaffiliationdoesnotalterouradherence mine,5-HT)[6,23,24],acetylcholine[4,13,25]anddopamine[6,20,24,26].Elevationofthe toPLOSONEpoliciesonsharingdataand materials. neurotransmitter5-HTresultedinactivationofcAMPresponseelement-bindingprotein (CREB)andsubsequentchangesintranscription,proteinphosphorylationandhistonemodi- fication[8,23,27].OtherresearchgroupshavesuggestedthatBacoparegulatepre-andpost- synapticproteins[9]andinducetheformationofnewdendrites[11,28].Theseproposed mechanismsarenotmutuallyexclusiveandthediscrepanciescouldbeattributedtoaselective biasinthetargetsthatwereinvestigatedbyeachresearchgroup. InordertobetterdefinethemolecularandcellularcomponentsofBacopaaction,wehave appliedadeepsequencingtechnique,RNA-Seq,toidentifythechangesinthetranscriptome uponBacopatreatment.Wehaveperformedbothatranscriptlevelandgenelevelanalysisto investigatethechangesingeneexpressioncausedbyBacopa.Theseexperimentshavesug- gestedunderlyingmechanismsofactionforBacopa,thebiologicalpathwaysalteredbythis plantextractandthepotentialupstreammediatorsfortheseprocesses. Materialsandmethods Cellculture,differentiationofSH-SY5YcellsandBacopatreatment Thehumanneuroblastomacellline,SH-SY5Y,waspurchasedfromtheAmericanTypeCul- tureCollection(ATCCCRL-2266).CellswereculturedinDMEM/F12(Sigma)supplemented in10%(v/v)fetalbovineserum(FBS,Gibco)and1%(v/v)penicillin/streptomycin(P/S,JR Scientific).ThismediumwillbereferredtoasCompleteMediumhenceforth.Subculturingwas performedaspermanufacturer’sinstructions(ATCC).Inbrief,astheSH-SY5Ycellsgrowasa mixtureoffloatingandadherentcells,carewastakentoensurethefloatingcellsinthe mediumwerecollectedandrecoveredbycentrifugation.Thesecollatedfloatingcellswouldbe combinedwithtrypsinizedadherentcellsandsubcultured.Cellswerealsopassagedlessthan threetimestoensurethatthecellsremainedneuroblast-like[29](Fig1Aand1C).Forexperi- mentsinvolvingundifferentiatedSH-SY5Ycells,theplatingdensitywas0.4x106cells/cm2.To differentiateSH-SY5Ycells,theywereplatedatadensityof0.5x106/cm2onculturesurfaces coatedwith10μg/mllaminin(Sigma)andmaintainedinCompleteMediumfor18h.After which,theyweremaintainedinserum-freeCompleteMedium.50nMofhumaninsulin-like growthfactor-I(IGF-1)(Sigma)wasaddedtopromotedifferentiation[30].48hafterthe switchtoserum-freeCompleteMediumandtheadditionofIGF-1,themediumwasreplen- ished.Bacopatreatmentwascarriedout72hafterthestartofdifferentiation.Undifferentiated anddifferentiatedcellsweretreatedwith3μg/mlBacopafor24hor10μg/mlBacopafor4h, orwithvehiclecontrols.Forallexperiments,weusedastandardizedextractofBacopa(CDRI- 08),containingnolessthan55%bacosideAandbacosideBasitsbioactivecomponentsthat wasextractedbyethanolextraction(LailaImpex,Vijaywada,India)[31,32]. Hydrogenperoxide(H O )toxicityassay 2 2 UndifferentiatedordifferentiatedSH-SY5Ycellswereexposedtodifferentconcentrationsof H O for24h.NumberoflivecellsweremeasuredusingtheLIVE/DEADassay(Invitrogen) 2 2 usinghigh-contentscreening(HCS)microscopyplatform(MetaXpress,Moleculardevices). PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 2/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Fig1.DifferentiationofSH-SY5YcellsusinglamininandIGF-1.SH-SY5Ycellswereplatedonlamininandgrownfor24hoursinDMEM/F12 supplementand10%FBS.Toinducedifferentiation,FBSwasremovedand50nmIGF-1wasadded;cellswereallowedtogrowfor72hours.(A) Differentialinterferencecontrast(DIC)imageoftheundifferentiatedcontrols.Redarrowsmarkedtheneuritesinundifferentiatedcellsthatwere characteristicforneuroblast-likecells.(B)DICimageofthedifferentiatedcells.Theincreaseinneuritelengthupondifferentiationwasmarkedout bythegreenarrowheads.(CandD)Toquantifythechangeinthelengthoftheneurites,twodaysintothedifferentiationprotocol,cellswere transfectedwithGFPcDNAandimagedonday3usingfluorescencemicroscopy.TransfectingwithGFPhighlightedtheneuritesamongthe confluentcelllayers,allowingforeasyquantification.(C)Anoverviewoftheundifferentiatedcontrols.Redarrowsmarkedouttheneuriteofeach GFPtransfectedcells.(D)Differentiatedcellsdisplayedlongneuritesasoutlinedbygreenarrowheads.(E)Theincreaseinthelengthofthe neuritesupondifferentiationwasstatisticallysignificant(unpairedt-test,****indicatesP-val<0.0001). https://doi.org/10.1371/journal.pone.0182984.g001 PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 3/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells High(10μg/ml)andlowconcentration(1μg/ml)ofBacopaweresupplementedduringthe additionofH O forinvestigationofneuroprotectiveeffectsofBacopa. 2 2 RNAsamplepreparation,libraryconstructionandRNAsequencing RNAwasharvestedfromtreatedSH-SY5YcellsusingtheNucleoSpinRNA/Proteinkit (Macherey-NagelGmbH).LibraryconstructionandRNAsequencingwereperformedbythe Duke-NUSGenomeBiologyFacility(DGBF).Briefly,2.2μgofRNAwassentforlibrarycon- struction.QualityofRNAwasanalyzedwiththeAgilentBioanalyzerandRNAwithRIN>9 wasused.Followingpoly-Aenrichment,recoveredRNAwasprocessedusingtheIllumina TruSeqRNASamplePreparationKitv2protocol(non-stranded)togenerateadaptor-ligated libraries.Atotalofsixsamplesweresequenced,obtainedfromundifferentiatedanddifferenti- atedSH-SY5Ycellstreatedwith(i)vehicle-treatedcontrol,(ii)3μg/mlBacopafor24h,and (iii)10μg/mlBacopafor4h.SamplesweresequencedusingtwolanesofanIllumina HiSeq2000sequencerusing76-bppaired-endreads. ComputationalanalysesofRNA-sequencingdata RNA-SeqdatawasmappedtothehumangenomeusingPartekFlow(version4.0.15.0406)and PartekGenomicsSuite(version6.15.0327).Aftertheadaptorsequencesweretrimmedaway, readsweremappedtotheHomosapiensgenome(hg38)withTopHat2(version2.0.8).Local alignmentwasperformedontheunalignedreadsfromTopHat2tothehumangenome(hg38) withBowtie2(version2.1.0).AlignedreadsfromtheTopHat2andBowtie2alignmentwere combinedinPartekFlow.Post-alignmentQA/QCwasperformedaftereachalignmentstep andalignedreadshadanaveragequalityPhredscoreabove30.Theuniquepairedreadswere usedforgeneexpressionquantification.Readswereassignedtoindividualtranscriptsofa genebasedontheExpectation/Maximization(E/M)algorithm[33].InthePartekGenomics Suitesoftware,theE/Malgorithmwasmodifiedtoacceptpaired-endreads,junctionaligned reads,andmultiplealignedreadsifthesearepresentinthedata.RNAexpressionwascalcu- latedasfragmentsperkilobaseoftranscriptpermillionmappedreads(FPKM)valuesofthe humanRefSeqgenesforpaired-endsequencing.Toidentifydifferentiallyexpressedgenes, Partek’sGeneSpecificAnalysis(GSA)algorithmwasused.Readcountsbetweensampleswere normalizedwiththeUpperQuantilemethodandanalysiswasperformedatthetranscript level.AcutoffvalueofmultimodalP<0.05andfoldchange>2or<-2wereset.Agene ontologyanalysiswasconductedusingPartekGenomicsSuite. Functionalclassscoringusinggene-setenrichmentandover- representationanalysis Toidentifybiologicalfunctionsaffectedbydifferentialgeneexpression,evidenceforfunc- tionalclassenrichmentinvolvingbiologicalpathwaysorgene-setswassoughtviatwoindepen- dentmethods.First,pathwayenrichmentanalysiswasconductedviatheGeneSetEnrichment Analysistoolusingthe“pre-ranked”option[34].Forthisanalysis,atotalof10744geneswith aFPKM(cid:21)5inatleast1samplewereincluded,andrankedbytheirfold-changeinexpression betweenthecontrolandBacopatreatedsamples.Therankedgene-listwasusedtoquerypath- waysfromGeneOntology-BiologicalProcessandGeneOntology-MolecularFunction, (downloadedfromtheMolecularSignaturesDatabase,MSigDB,[35],aswellascustompath- ways(Reactomepathwaysplususer-definedgene-setsforbrain-specificfunctions)forstatisti- callysignificantenrichmentofhigherorlowerrankedgenes.Significanceestimateswere adjustedformultipletestingviathefalsediscoveryrate(FDR). PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 4/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Over-representationanalysis(ORA)ofbiologicalfunctionsandputativeupstreamregula- torswascarriedoutbysubjectingapre-filteredlistof576differentiallyexpressedgenes (FPKM(cid:20)5inatleast1sampleandabsolutefold-change(cid:21)1.5)toQIAGEN’sIngenuityPath- wayAnalysistool(IPA,QIAGENRedwoodCity,https://www.qiagenbioinformatics.com/ product-login/).First,referencegene-setscorrespondingto‘biologicalfunctions’(asdefined intheIngenuityKnowledgeBase),wereanalyzedviaFisher’sexacttestforstatisticallysignifi- cantover-representationinthelistofdifferentiallyexpressedgenes.Additionally,predictions ofchangesintheactivitystatusof‘upstreamregulators’(specifically,transcriptionfactors), thatcouldputativelyexplaintheobservedgeneexpressionchangesduetoBacopatreatments, wasalsocarriedout.AnORAwasfirstperformedtodeterminewhetheranupstreamregulator wasenrichedfordifferentialexpressionofitstargetgenes(thelistofregulatorsandtheirtarget geneswere,again,obtainedfromtheIngenuityKnowledgeBase).Theoverallactivationor inhibitionstatusoftheregulatorwastheninferredfromthedegreeofconsistency(up-or down-regulation)intheexpressionpatternsofitstargetgenes,expressedasaz-score.Regula- torswithz(cid:21)2orz(cid:21)−2wereconsideredtobeactivatedorinhibited,respectively. cDNAsynthesisandquantitativeReal-TimePolymeraseChainReaction (qRT-PCR) RNAwasharvestedusingtheNucleoSpinRNA/Proteinkit(Macherey-NagelGmbH).The amountofRNAwasmeasuredspectrophotometricallyusingaNanodropND-1000Spectro- photometer.cDNAwasgeneratedfrom2μgofRNAusingtheiScriptcDNAsynthesiskit(Bio- RadLaboratories).Randomhexanucleotideswereannealedfor5minat25˚C.cDNAsynthesis wasperformedfor30minat42˚C,followedbyanenzymeinactivationstepfor5minat85˚C. cDNAwasstoredat-20˚Cuntiluse.1μlofthecDNAreactionmixwasusedforqRT-PCR, whichwasperformedusingiQSYBRgreenreagents(Bio-RadLaboratories)ontheiQ5Multi- colorReal-TimePCRDetectionSystem(Bio-RadLaboratories)withthefollowingPCRprofile: 95˚Cfor3min,40cyclesof95˚Cfor10sand55˚Cfor30s.AfterthecompletionofthePCR, meltcurveanalysiswasperformedusingthefollowingparadigm:95˚Cfor1min,55˚Cfor1 minfollowedbyrampingupthetemperaturefrom55˚Cto95˚C.RPL19wasusedasacontrol. Results CharacterizationofSH-SY5Ycells ThegoaloftheseexperimentswastocharacterizetheeffectsofBacopaonfunctionalproper- tiesandgeneexpressionprofilesofSH-SY5Yhumanneuroblastomacells.Inthepresenceof serum,undifferentiatedSH-SY5Ycellscanbepropagatedindefinitely,whiletheycanbemade toterminallydifferentiatebywithdrawingserum,platingonaproperlycoatedsurfaceand additionofdifferentiatingfactors.SH-SY5Ycells(passagenumber27,www.atcc.org)weredif- ferentiatedbyplatingthemonlaminin-coatedcoverslips,usingaprotocoloptimizedby Dwaneetal[30],whichconsistedofremovingfetalbovineserum(FBS)andadding50nM InsulinGrowthFactor1(IGF-1).Cellsshowedadifferentiatedneuronalphenotype(forma- tionofextensiveneurites)after3–5days(Fig1B).Inordertoobtainabettervisualizationof theindividualcells,wetransfectedthecultureswithacDNAencodingGreenFluorescentPro- tein(GFP)andusedfluorescencemicroscopytodocumentthedifferentiation(Fig1Dand 1E).Fig1illustratestheresultsofdifferentiationonthemorphologyofSH-SY5Ycells.Upon differentiation,therewasasignificant3.4foldincreaseintheneuritelengthintheSH-SY5Y cells(undifferentiatedcells:19.4μm;differentiatedcells:66.2μm,studentt-test,P- val=0.0001)(Fig1E). PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 5/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells RNA-Seqanalysis InordertounderstandthechangesingeneexpressionlevelscausedbyBacopa,weperformed acomprehensiveRNA-SeqanalysisforbothundifferentiatedanddifferentiatedSH-SY5Yneu- roblastomacells.Twodifferentconcentrationsandtreatmenttimeswereused:10μg/mlfor4 hoursand3μg/mlfor24hours.Theseconcentrationsweredeterminedinpilotexperimentsto bethehighestconcentrationsthatwerenotdeleterioustothecells.Vehicle(DMSO)wasused asacontrolfortheBacopaeffect.Inaddition,weevaluatedtheeffectofdifferentiationitself. Foreachcondition,thesequenceof50millionmRNAfragments(“reads”)wasobtained whichwerethenmappedtothehumangenome,asdescribedintheMethodssection,resulting inarelativeabundanceforallmRNAsexpressedatareasonablelevel.Foreach“treatment”,a listofdifferentiallyexpressedmRNAswasgenerated,usingaP-valuesmallerthan0.05andan absolutefold-changeofatleast2.Table1summarizestheresults. Effectofdifferentiation DifferentiationofSH-SY5Ycellswasaccomplishedbygrowingthemonlamininandreplacing serumwithIGF-1.Cellsshowedadifferentiatedphenotype(formationofextensiveneurites) after3–5days(Fig1B,1Dand1E).TheRNA-Seqanalysisdetected31,500differenttranscripts inSH-SY5Ycells.Duetoalternativesplicing,thenumberofdistinctmRNAsinacellistypi- callylargerthanthenumberofgenes(~23,000)inthehumangenome.Thedifferentiationpro- tocolresultedinachangeof502mRNAlevels,ofwhich78couldbeclassifiedastranscribed from‘neuronal’genes(S1Table).Theresultsindicatedthat(1)ourdifferentiationprotocol waseffectiveinalteringthegeneexpressionprofiletowardsamoreneuronalphenotype,and (2)theRNA-SeqapproachcanbeusedtoidentifychangesinmRNAlevelsinanun-biased mannerandatagenomewidescale. EffectofBacopatreatment:Individualtranscriptlevelanalysis Table1summarizestheeffectoffourdifferentBacopatreatmentprotocols(2concentrations/ durationsinundifferentiatedanddifferentiatedSH-SY5Ycells)onthemRNAprofileofthe neuroblastomacells.The4-hourtreatmentwithBacopaalteredtheexpressionofmore mRNAsthanthe24-hourBacopatreatment:57and66vs.37and29alteredmRNAsinundif- ferentiatedanddifferentiatedcells,respectively(Table1).Thisindicatedthattheeffectof Bacopaongenetranscriptionseenafter4hourssubsidesafteronedayformanyoftheaffected transcripts.4hoursofBacopaondifferentiatedcellswasmosteffective,with66mRNAsbeing alteredatleast2-fold(Table1).Thisdatasetwasthereforeselectedforfurtheranalysis.Agene ontologyanalysiswasconductedusingPartekGenomicsSuite.Fig2illustratestheresults, Table1. NumberofmRNAsalteredbydifferentiationandBacopatreatment. Effectof #mRNAswithfoldchange>2 #neuronalmRNAs Differentiation(laminin,IFG-1) 502 78 10μg/mlBacopa4hours(Undifferentiated) 57 1 3μg/mlBacopa24hours(Undifferentiated) 37 4 10μg/mlBacopa4hours(Differentiated) 66 20 3μg/mlBacopa24hours(Differentiated) 29 4 WeconsideredmRNAlevelstobealterediftheP-valuewassmallerthan0.05andtheabsolutevalueofthefoldchangewaslargerthan2.Fourhoursof Bacopaondifferentiatedcellswasmosteffective(highlightedinboldanditalics). https://doi.org/10.1371/journal.pone.0182984.t001 PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 6/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Fig2.ResultsofthegeneontologyanalysisbyPartekGenomicsSuite.Thebargraphsindicatethepercentageoftranscripts thatbelongtoBiologicalProcesses(blue),CellularComponents(red)andMolecularFunctions(green)thatweremostaffectedby Bacopatreatment. https://doi.org/10.1371/journal.pone.0182984.g002 listingthebiologicalprocesses,cellularcomponentsandmolecularfunctionsaffectedby Bacopatreatment.Manyoftheaffectedbiologicalprocessesreferredtofunctionsthatwereof criticalimportanceinthecentralnervoussystem.Table2summarizesthemRNAsalteredby Bacopatreatmentencodedbygeneswithaneuronalfunction.Themoststrikingfindingwas theNeuroplastingene(NPTN),becauseasinglenucleotidepolymorphism(SNP)intheNeu- roplastinlocusassociateswithcorticalthicknessandintellectualabilityinadolescents[36]. Neuroplastinisasynapticglycoproteininvolvedinlong-termpotentiation(LTP)inhippo- campalCA1synapsesthatmodulatesneuritogenesisandneuronalplasticity[37,38]. EffectofBacopatreatment:Genelevelanalysis Theanalysisdescribedabovewasbasedonmappingthereadstoindividualtranscriptsofthe humangenome(seeMaterialsandmethods).Becauseoftheextensivealternativesplicingseen formanygenes,aprocessthatismostprominentinthebrain,mappingthereadsisadifficult processandboundtobeerror-prone.Wehavethereforeusedanadditionalanalysis,whichis morerobust,inwhichthereadsmappedtoallexonsbelongingtoagenewerecombinedto provideagenelevelstatistic.SeveraladditionalgenesregulatedbyBacopawereidentifiedthis way,assummarizedinTable3. PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 7/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Table2. SummaryofneuronalgeneswhosemRNAswerealteredbyBacopatreatmentofSH-SY5Ycells. Gene Genename Fold Function Symbol change HNRNPC HeterogeneousnuclearribonucleoproteinC 19.7 PromotesAPPtranslationbycompetingwithFMRPforAPPmRNA recruitmenttoPbodies CIB2 Calciumandintegrinbindingfamilymember2 6.7 RoleinCa2+homeostasisandCa2+regulationinthemechano-transduction process;Mutationscausedeafness NPTN Neuroplastin 6.6 Regulationoflong-termneuronalsynapticplasticity,cytosolicCa2+ion concentration,neuronprojectiondevelopment;SNPsassociatedwith cognitiveabilitiesinadolescents COMMD6 COMMDomainContaining6 6.4 NF-KappaBbinding;Regulatestranscriptionfactoractivity,geneexpression NDUFA5 NADHDehydrogenase1AlphaSubcomplex5 (4.7) Mitochondrialtransport CHAC1 ChaCGlutathione-SpecificGamma- 4.0 NegativeregulatorofNotchsignalingpathwayinvolvedinembryonic Glutamylcyclotransferase1 neurogenesis;Promotesneurogenesisinembryos AP2S1 Adaptor-RelatedProteinComplex2,Sigma1 3.8 Synaptictransmission;RegulatesEGFR,TRKreceptor,ephrinreceptor Subunit pathway KCNMA1 KChannel,CaActivatedLargeConductanceM (3.3) Regulationofmembranepotential;Synaptictransmission Alpha1 NGFR NerveGrowthFactorReceptor 3 Mediatescellsurvivalandcelldeathofneuralcells;Necessaryforcircadian oscillationinsuprachiasmaticnucleus STRN3 Striatin-3 2.6 GlutamateregulationofdopamineD1Areceptorsignaling PRKACB ProteinKinase,CAMP-Dependent,Catalytic, (2.6) MediatessignalingthroughcAMP;Involvedinneuronalstructureand Beta signaling LDHA LactateDehydrogenaseA (2.5) Substantianigradevelopment MTMR2 MyotubularinRelatedProtein2 2.3 MutationsresultinCharcot-MarieToothdiseasetype4B,anautosomal recessivedemyelinatingneuropathy VCL Vinculin 2.3 Involvedinregulationofactincytoskeleton,axonandneuronprojection extension;Hasanegativeregulationoncellmigration WDR1 WDRepeatDomain1 2.3 Involvedinsensoryperceptionofsound,regulationofoligodendrocyte differentiationorgliogenesisandneurogenesis DBI DiazepamBindingInhibitor(GABAReceptor (2.3) ModulatessignaltransductionatGABA receptors;Displacesdiazepam A Modulator,Acyl-CoABindingProtein) fromthebenzodiazepinerecognitionsiteinGABA receptor A EFNB2 Ephrin-B2 (2.3) Mediatedevelopmentofthenervoussystem;Crucialformigration,repulsion andadhesionduringneuronaldevelopment ACTB Actin,Beta 2.2 Involvedinaxonogenesis,axonguidance,neuronprojection morphogenesis,substantianigradevelopment,ATP-dependentchromatin remodeling,ephrinreceptorsignalingpathway ACTG1 ActinGamma1 2.2 AssociatedwithDFNA2-/26,asubtypeofautosomaldominantnon- syndromicsensorineuralprogressivehearingloss;InvolvedinRassignaling pathway,axonalguidance SLC38A1 SoluteCarrierFamily38,Member1 2.2 Glutaminetransporter,precursorforthesynaptictransmitter,glutamateand GABA;Involvedinsynaptictransmissionandneurotransmitterreuptake STMN4 Stathmin-Like4 (2.2) Involvedinneuronprojectiondevelopment,microtubuledepolymerization, neuronalplasticity,rapidlyinducedafterseizureorLTP CALR Calreticulin 2.1 MajorCa2+-bindingproteininthelumenoftheER;Essentialforintegrin- mediatedsignalingandcelladhesion SLC1A4 SoluteCarrierFamily1(Glutamate/NeutralAmino 2.1 AssociatedwithHartnupdisorder;Chloridechannelactivity;Transporterfor AcidTransporter),Member4 alanine,serine,cysteineandthreonine,sodiumdependent KLHL24 Kelch-LikeFamilyMember24 (2.1) Reduceskainatereceptor-mediatedcurrentsinhippocampalneurons ATF4 ActivatingTranscriptionFactor4 2 Transcriptionalactivator;ProtectsagainstneuronaldeathinParkinson’s disease;Involvedinneurodegeneration;Mayconstrainlong-termsynaptic changesandmemoryformation NRCAM NeuronalCellAdhesionMolecule (2.0) Involvedinneuron-neuronadhesion;Promotesdirectionalsignalingduring axonalconegrowth STMN1 Stathmin1 (2.0) Requiredforaxonformationduringneurogenesis;Involvedinthecontrolof learnedandinnatefear (Continued) PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 8/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Table2. (Continued) Gene Genename Fold Function Symbol change XRCC6 X-RayRepairComplementingDefectiveRepairin (2.0) Involvedinbraindevelopment;Positiveregulationofneurogenesis ChineseHamsterCells6 https://doi.org/10.1371/journal.pone.0182984.t002 ValidationoftheRNA-sequencingresults:qRT-PCR Next,wevalidatedtheRNA-SequencingresultsusingqRT-PCRexperimentsforasubsetof genes.Fig3summarizestheresultsbyshowingtheabsolutevalueofthefoldchangeproduced byBacopatreatment.Inthecaseofgeneswithalternativelysplicedtranscripts,PCRprimer pairsweredesignedthatwereuniqueforthemRNAisoformthatwasalteredbyBacopa.In somecases,thisprovedtobehard,sincetheexonthatwasuniqueforthealteredtranscript wasveryshort.AcaseinpointisNeuroplastin,whichhasfourmRNAvariants,oneofwhich isaffectedbyBacopa(NPTN_D).Thedistinguishingfeatureoftheaffectedvariantisthe absenceofexon2andthatexon7isshortenedby12nucleotides.Wewereabletovalidatethe Table3. GenesregulatedbyBacopaidentifiedbygene-levelanalysisoftheRNA-Seqdata. Gene Genename Fold Function Symbol Change HBA2 Hemoglobin,Alpha2 405 Oxygen-transportmetalloproteinintheredbloodcells HBB Hemoglobin,Beta 370 Oxygen-transportmetalloproteinintheredbloodcells HBA1 Hemoglobin,Alpha1 292 Oxygen-transportmetalloproteinintheredbloodcells ANKRD1 AnkyrinRepeatDomain1 21.7 Transcriptionfactorinvolvedindevelopmentandunderconditionsof stress SLC7A11 SoluteCarrierFamily7Member11 7.5 Transporterthatantiportsglutamateforcysteine SERPINE1 SerpinPeptidaseInhibitor,CladeE 6.8 Serineproteaseinhibitorthatfunctionsastheprincipalinhibitoroftissue plasminogenactivatorandurokinase WNT8B Wingless-TypeMMTVIntegrationSiteFamily, 6.8 Wntisoformspecificforthedevelopingbrain Member8B HIST1H4K HistoneCluster1,H4k 5.3 HistoneH4isoform HIST1H4J HistoneCluster1,H4j 5.2 HistoneH4isoform CCL2 Chemokine(C-CMotif)Ligand2 4.8 Recruitsmonocytes,memoryTcells,anddendriticcellstositesof inflammationproducedbyinjuryorinfection CHAC1 ChaCGlutathione-SpecificGamma- 4.5 Proapoptoticcomponentoftheunfoldedproteinresponse;Downstreamof Glutamylcyclotransferase1 theATF4-ATF3-CHOPcascade NTS Neurotensin 4.4 Neuropeptideimplicatedintheregulationofhormonerelease;Has interactionwiththedopaminergicsystem ANGPTL4 Angiopoietin-LikeProtein4 4.0 Inducedunderhypoxicconditions;Serumhormonedirectlyinvolvedin regulatinglipidmetabolism PTPRH ProteinTyrosinePhosphatase,ReceptorType, (3.8) Ubiquitouslyexpressed;Upregulatedingastrointestinalcancers H TXNIP ThioredoxinInteractingProtein (3.8) Glucocorticoid-regulatedprimaryresponsegeneinvolvedinmediating glucocorticoid-inducedapoptosis YPEL4 Yippee-Like4(Drosophila) (3.6) Nuclearprotein;ActivatesElk-1intheMAPKsignalingpathway;Possible functionincelldivision CNN2 Calponin2 3.5 Actin-bindingproteinimplicatedincytoskeletalorganization RAPGEF4 Rapguaninenucleotideexchangefactor4 (3.0) EPAC2;Mayregulatesynapticplasticity STON1 Stonin1 (3.0) Componentoftheendocyticmachinery FMN1 Formin1 (3.0) Roleintheformationofadherensjunctionandthepolymerizationoflinear actincables https://doi.org/10.1371/journal.pone.0182984.t003 PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 9/21 EffectofBacopaongeneexpressioninhumanneuroblastomacells Fig3.AbsolutevaluesofFoldChange(absFC)causedbyBacopatreatment.RT-PCRwasperformedonundifferentiatedcellsand differentiatedcellswhichweretreatedwithvehicle(DMSO)orwithBacopaforeither4h(blue)or24h(orange).Thegrayareaindicatedan absFCvaluesmallerthan1.Genesmarkedwith*wereresultsfromthetreatmentonundifferentiatedcells.(1)NPTN_Aand(2)NPTN_A wereresultsgeneratedfrom2setsofprimersprimingforNPTNtranscriptA. https://doi.org/10.1371/journal.pone.0182984.g003 effectsofBacopaonthetranscriptsidentifiedbythegene-levelanalysis(ANKRD1,SLC7A11, CHAC1,TXNIP,YPEL4andSTON1)(Table3).However,forthemRNAsforwhichonlyone orafewofthealternativelysplicedvariantswereaffectedbyBacopa,thevalidationwasless successful:theeffectswereeithermuchsmallerthanthoseseenintheRNA-Seqanalysis (HBA1andHBA2)(Table3)ortherewasnomeasurableeffect(NPTN_D)(Table2). PLOSONE|https://doi.org/10.1371/journal.pone.0182984 August23,2017 10/21