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Prevalence of Propionibacterium acnes in Intervertebral Discs of Patients Undergoing Lumbar PDF

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Preview Prevalence of Propionibacterium acnes in Intervertebral Discs of Patients Undergoing Lumbar

RESEARCHARTICLE Propionibacterium acnes Prevalence of in Intervertebral Discs of Patients Undergoing Lumbar Microdiscectomy: A Prospective Cross-Sectional Study ManuN.Capoor1,3*,FilipRuzicka2,TanaMachackova3,RadimJancalek4,MartinSmrcka5, JonathanE.Schmitz6,MarketaHermanova7,JiriSana3,ElleniMichu3,JohnC.Baird3, FahadS.Ahmed3,KarelMaca5,RadimLipina8,ToddF.Alamin9,MichaelF.Coscia10,Jerry a11111 L.Stonemetz11,TimothyWitham12,GarthD.Ehrlich13,14,15,ZiyaL.Gokaslan16, KonstantinosMavrommatis17,ChristofBirkenmaier18,VincentA.Fischetti1, OndrejSlaby3* 1 LaboratoryofBacterialPathogenesisandImmunology,RockefellerUniversity,NewYork,NY,United StatesofAmerica,2 DepartmentofMicrobiology,FacultyofMedicine,Masarykuniversity,St.Anne’sFaculty Hospital,Brno,CzechRepublic,3 DepartmentofMolecularOncology,CentralEuropeanInstituteof Technology(CEITEC),MasarykUniversity,Brno,CzechRepublic,4 DepartmentofNeurosurgery, OPENACCESS St.Anne’sUniversityHospital,MasarykUniversity,Brno,CzechRepublic,5 DepartmentofNeurosurgery, UniversityHospitalBrno,MasarykUniversity,Brno,CzechRepublic,6 DepartmentofPathology, Citation:CapoorMN,RuzickaF,MachackovaT, MicrobiologyandImmunology,VanderbiltUniversitySchoolofMedicine,Nashville,TN,UnitedStatesof JancalekR,SmrckaM,SchmitzJE,etal.(2016) America,7 1stDepartmentofPathologicalAnatomy,St.Anne’sUniversityHospital,MasarykUniversity, PrevalenceofPropionibacteriumacnesin Brno,CzechRepublic,8 DepartmentofNeurosurgery,UniversityHospitalOstrava,OstravaUniversity, IntervertebralDiscsofPatientsUndergoingLumbar Ostrava,CzechRepublic,9 DepartmentofOrthopedicSurgery,StanfordUniversityMedicalCenter, StanfordUniversity,Stanford,CA,UnitedStatesofAmerica,10 DepartmentofOrthopedicSurgery, Microdiscectomy:AProspectiveCross-Sectional OrthoIndyHospital,Indianapolis,IN,UnitedStatesofAmerica,11 DepartmentofAnesthesia,TheJohns Study.PLoSONE11(8):e0161676.doi:10.1371/ HopkinsHospital,Baltimore,MD,UnitedStatesofAmerica,12 DepartmentofNeurosurgery,TheJohns journal.pone.0161676 HopkinsHospital,Baltimore,MD,UnitedStatesofAmerica,13 CenterforGenomicSciences,Drexel Editor:HolgerBrüggemann,AarhusUniversitet, UniversityCollegeofMedicine,Philadelphia,Pennsylvania,UnitedStatesofAmerica,14 Departmentof MicrobiologyandImmunology,DrexelUniversityCollegeofMedicine,Philadelphia,Pennsylvania,United DENMARK StatesofAmerica,15 DepartmentofOtolaryngologyHeadandNeckSurgery,DrexelUniversityCollegeof Received:July18,2016 Medicine,Philadelphia,Pennsylvania,UnitedStatesofAmerica,andInstituteofMolecularMedicineand InfectiousDisease,DrexelUniversityCollegeofMedicine,Philadelphia,PA,UnitedStatesofAmerica, Accepted:August9,2016 16 DepartmentofNeurosurgery,TheWarrenAlpertMedicalSchoolofBrownUniversity,RhodeIsland Hospital,Providence,RI,UnitedStatesofAmerica,17 CelgeneCorporation,InformationKnowledgeand Published:August18,2016 Utilization,SanFrancisco,CA,UnitedStatesofAmerica,18 DepartmentofOrthopedics,PhysicalMedicine Copyright:©2016Capooretal.Thisisanopen &Rehabilitation,UniversityofMunich(LMU),Munich,Germany accessarticledistributedunderthetermsofthe *[email protected](OS);[email protected](MNC) CreativeCommonsAttributionLicense,whichpermits unrestricteduse,distribution,andreproductioninany medium,providedtheoriginalauthorandsourceare credited. Abstract DataAvailabilityStatement:Allrelevantdataare withinthemanuscript. Funding:DiscitisDxprovidedsupportintheformofa Background researchgrantwhichwasusedtopayforculturing TherelationshipbetweenintervertebraldiscdegenerationandchronicinfectionbyPropio- andPCRreagentsandmaterials.NeitherDiscitiDX, Inc.noranyothercommercialorganizationprovided nibacteriumacnesiscontroversialwithcontradictoryevidenceavailableintheliterature. anysupportintheformofsalariesforauthorsanddid Previousstudiesinvestigatingtheserelationshipswereunder-poweredandfraughtwith nothaveanyroleinthestudydesign,datacollection methodicaldifferences;moreover,theyhavenottakenintoconsiderationP.acnes’abilityto andanalysis,decisiontopublish,orpreparationof formbiofilmsorattemptedtoquantitatethebioburdenwithregardtodeterminingbacterial themanuscript.Thespecificrolesoftheseauthors arearticulatedinthe‘authorcontributions’section. counts/genomeequivalentsascriteriatodifferentiatetrueinfectionfromcontamination.The PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 1/12 P.acnes'PrevalenceinHerniatedDiscs CompetingInterests:Theauthorshavereadthe aimofthisprospectivecross-sectionalstudywastodeterminetheprevalenceofP.acnesin journal'spolicyandtheauthorsofthismanuscript patientsundergoinglumbardiscmicrodiscectomy. havethefollowingcompetinginterests:MNC,FSA, JLS,CB,OS,JES,K.Mavrommatis,andVAFhave stockownershiporoptionsinDiscitisDX,Inc.There MethodsandFindings arenootherfinancialornon-financialcompeting Thesampleconsistedof290adultpatientsundergoinglumbarmicrodiscectomyforsymp- interests.Thisdoesnotaltertheauthors'adherence toPLOSpoliciesonsharingdataandmaterials. tomaticlumbardischerniation.Anintraoperativebiopsyandpre-operativeclinicaldata weretakeninallcases.Onebiopsyfragmentwashomogenizedandusedforquantitative anaerobiccultureandasecondwasfrozenandusedforreal-timePCR-basedquantifica- tionofP.acnesgenomes.P.acneswasidentifiedin115cases(40%),coagulase-negative staphylococciin31cases(11%)andalpha-hemolyticstreptococciin8cases(3%).P. acnescountsrangedfrom100to9000CFU/mlwithamedianof400CFU/ml.Thepreva- lenceofintervertebraldiscswithabundantP.acnes((cid:1)1x103CFU/ml)was11%(39cases). Therewassignificantcorrelationbetweenthebacterialcountsobtainedbycultureandthe numberofP.acnesgenomesdetectedbyreal-timePCR(r=0.4363,p<0.0001). Conclusions Inalargeseriesofpatients,theprevalenceofdiscswithabundantP.acneswas11%.We believe,disctissuehomogenizationreleasesP.acnesfromthebiofilmsothattheycanthen potentiallybecultured,reducingtherateoffalse-negativecultures.Further,quantification studyrevealingsignificantbioburdenbasedonbothcultureandreal-timePCRminimizethe likelihoodthatobservedfindingsareduetocontaminationandsupportsthehypothesisP. acnesactsasapathogeninthesecasesofdegenerativediscdisease. Introduction Propionibacteriumacnes(P.acnes)isafacultativeanaerobic,Gram-positive,slow-growing,fas- tidiousbacteria[1,2]prevalentonhumanskinandsebaceousductsaspartofthenormalflora [3,4,5]andisimplicatedinthedevelopmentofacnevulgaris[6]aswellaspostoperativeand device-relatedinfections[7].P.acneshavealsobeenidentifiedintheoralcavity,gastrointesti- naltract,genitourinarytract,eye(conjunctiva),andexternalearcanal[1].P.acnesmayplaya roleinotherconditions,includingprostatitis[8],SAPHO[9],sarcoidosis[10],anddegenera- tivediscdisease[11]. Thepioneeringstudypublishedin2001byStirlingetal.inLancet,reportedthat53%ofthe patientswithseveresciaticahadGram-positiveanaerobicmicroorganismsintheirdisctissue ofwhich84%wereP.acnes[12].ConsideringthepotentialclinicalconsequencesofaP.acnes infectionasanetiologicalfactorindegenerativediscdisease,thesefindingsareindicativeof potentiallysignificantsimilaritiestothediscoveryofHelicobacterpyloriinvolvementinpatho- genesisofpepticulcersandtheshiftitledtointhewaypepticulcersaretreated[13].Subse- quently,severalindependentstudieshavedemonstratedthepresenceofinfectedextrudeddisc tissuefromfirst-timedischerniations,withP.acnesbeingthemostcommonlyinvolvedorgan- ism[14–18].Accordingtoameta-analysisofthesestudiesfrom2015,P.acneswasthemost prevalentbacteriaindisctissue,withthepooledestimateoftheproportionwithpositivesam- plesbeing34%[19].Morerecently,thefirstexperimentalevidencewasprovidedshowingthat P.acneshastheabilitytoinducediscdegenerationinarabbitmodel[20].Otherstudies, PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 2/12 P.acnes'PrevalenceinHerniatedDiscs however,reportedveryloworzeroprevalenceofbacterialinfectioninsamplesfrompatients withlumbardischerniation,quotingcontaminationasthepredominantsource[21–23]. Contributingtothislackofconsensus,significantmethodicaldifferencesexistamongstud- ies.Themostnotableofwhichisthelackoflaboratoryproceduresthattakeintoaccountapos- siblebiofilmmodeofgrowthassociatedwithP.acnesinfection.Thistranslatesinto inconsistenciesinregardtotissuehomogenizationprocedurestobreakupbiofilmaggregates, leadingtonegativecultureresults.Asaconsequence,P.acnespositivitywaslikelyunderesti- matedinsomeofthepreviousstudies[21,23].Noneofthestudiesimplementedquantitative cultureorreal-timePCR-basedquantificationofP.acnesgenomes.Webelievethatquantita- tionofthebacterialbioburdenisanimportantcriterionthatcancontributetodiscrimination betweentrulyinfectedandskin-contaminatedcases.Thus,alackofquantitativemethodsto identifyP.acnescouldhaveledtooverestimatingthepositivityratesinpreviousstudies.These methodicalweaknessestogetherwiththesmallsamplesizes(onlyonestudyenrolledmore than100patientsforbacterialculture[23])haveleftthesestudiesunderpowered,withlimited applicabilityoftheirresultstowardsclinicaldecision-makingoranydefinitiveconclusions. Inthisprospectivecross-sectionalstudyonthecurrentlylargestseriesofpatientsundergo- ingmicrodiscectomyforlumbardischerniation,weimplementeddisctissuehomogenization, quantitativemicrobiologicculture,real-timePCR-baseddetectionofP.acnesgenomes,and proceduralDNAcontaminationcontrolstodetermineP.acnescountsindisctissuesamples andevaluatedtheprevalenceofintervertebraldiscswithanabundanceofP.acnes. Methods Studydesignandpatients BetweenMay2015andDecember2015,adultsscheduledformicrodiscectomyforsymptom- aticlumbardischerniationatUniversityHospitalBrno(Brno,CzechRepublic)andSt.Anne’s UniversityHospital(Brno,CzechRepublic)wereprospectivelyscreenedforpotentialpartici- pationinthiscross-sectionalstudy.Inclusioncriteriaincluded:lumbarorlumbosacralradicu- lopathywithorwithoutsensorydeficitsbutwitheitheramatching,clinicallyrelevantmotor deficitincorrelatinglumbarorsacralnerverootdistributions(seeimagingcriteria)orwith radicularpain(sciaticaorfemoralgia)thatwasintractablebyconservativemeans;matching physicalexaminationfindingsincludingpositivestraightlegraisetest,dermatomalsensory deficits,myotomalmotordeficitsand/oradiminisheddeeptendonreflexes;currentmagnetic resonanceimagingorcomputedtomographyimagingofthelumbosacralspineshowingafree nucleuspulposussequestrationoradischerniation/protrusioninadistributioncorrelating withtheclinicallyaffectednerverootsandwiththephysicalexamination.Exclusioncriteria included:coexistentinfectionorimmunologicallycompromisedconditions;corticosteroidor antibioticsuseinthemonthbeforesurgery;trauma;unknownradiographicmass;diagnosisof inflammatoryarthritisorotherrheumatologicdiseases.Thefollowingepidemiologicaland clinicaldatawerecollected:Gender,age,intervertebralsegmentinvolved,typeofherniation, prevalenceofpreviousspinalsurgeries,priorepiduralsteroidinjections,anddevelopmentof post-operativediscitis.Awritteninformedconsentwasobtainedfromeachpatient.Thestudy wasapprovedbytheInstitutionalReviewBoardsofUniversityHospitalBrnoandSt.Anne’s UniversityHospitalBrno. Collectionofintraoperativesamples Thesurgicalsitewasscrubbedwithtriplepreparationofpovidoneiodineanddrapedusing standardsteriletechnique.Standardperioperativeantibioticsweregivenbeforetheskininci- sioninallcases.Cefazolinwasthestandardantibioticgiveninmostcases.Inpenicillin-allergic PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 3/12 P.acnes'PrevalenceinHerniatedDiscs patients,eithervancomycinorclindamycinwasadministered.Thepreciselocationfortheskin incisionwasguidedbyintraoperativefluoroscopyandaposteriormidlineapproachusing sharpdissectionandelectrocauterywasperformed.Afterplacementofaself-retainingretrac- tor(Caspartype)andunderanoperatingmicroscope,ligamentumflavumwasresectedas requiredbymeansofPenfielddissectorsandKerrisonrongeurs.Thedischerniationwas exposedbygentleretractionofthetraversingnerverootandthenremovedtogetherwiththe remnantloosefragmentsofthenucleuspulposusinthediscspaceneartheannulardefect.All tissuesampleswerehandledinsuchawayastominimizetheircontamination,retainedina closedsterilesamplecup,andthenpassedofftothefieldforlabelingandtransporttothe DepartmentofMicrobiologyatSt.Anne’sUniversityhospital(Brno,CzechRepublic),where thedisctissuessamplesfrombothcenterswerefurtheranalyzed.Thesamplesizeswere approximately3x3x5-10x5x5mmandnotmeasuredaccuratelyasweattemptedtoobtainas muchmaterialasthepossiblefromthesurgicalspecimen.Sampleswerenotfrozenpriorto processingandculturewasestablishedwithin2to4hourspost-surgery. Microbiologicalculture Freshdisctissuesampleswerecutintosmallerfragmentsusingasterile,individuallypackaged, gamma-irradiatedscalpel;and,asterile,gamma-irradiatedpetridish.Oneofthesefragments wasplacedintoa2mLmicrocentrifugeDNA-freetubeandstoredat-80°Cuntilprocessedfor P.acnesDNAanalysis.Tissueprocessingandhomogenizationwascarriedoutinasterilepestle andmortarwithsterilequartzsand(sizeparticle0.1–0.5mm;Penta,CzechRepublic)and salinesolutioninasepticconditions,inaclass2biologicalsafetycabinet.Thehomogenizedtis- suesampleswereinoculatedontoWilkinsChalgrenAnaerobicAgar(HiMediaLaboratories, India)with7%ofsheep’sbloodandvitaminK.Inoculatedplateswereincubatedanaerobically (80%nitrogen,10%CO and10%H )inanAnaerobicWorkStation(RuskinnTechnology, 2 2 UK)at37°Cfor14daysandassessedforbacterialgrowth.Thequantityofbacteriainthesam- plewasexpressedascolonyformingunits(CFU)in1mlofthehomogenate.Identificationof bacteriawascarriedoutbiochemicallyusingtheRapidANAIISystem(Remel,USA). Quantitativereal-timePCR Frozentissuesampleswerethawed(medianwetweightwas130mg,range20–180mg),cut intosmallfragmentsandtransferredtoasterile2mLmicrocentrifugetubebyuseofnewly openedsterilesetsofneedle,scalpelandtweezers.Smallfragmentsofthetissuesampleswere furthersuspendedin500μlofATLbuffer(Qiagen,Germany)with50μlofproteinaseK(20 mg/ml)(Qiagen)anddigestedat56°Cand650rpminathermomixerovernight.Toeachsetof thesamplesthatwereprocessedinparallel,weusedatubewithsterilewaterasalaboratory contaminationcontroltofollowtheentirelaboratoryprocessfromdigestionofthetissueand DNAisolationtoreal-timePCRanalysis.DNAwasextractedbyuseoftheQIAampUCPPath- ogenMiniKit(Qiagen)asdescribedinthemanufacturer’sinstructions.Concentrationof DNAweremeasuredspectrophotometricallyusingaNanodrop2000(Thermofischer,USA); orwithfluorescentdyeandaQubit3.0fluorometer(LifeTechnologies,USA)forsampleswith DNAconcentrationslessthan5ng/μl.Apreviouslydescribedreal-timePCRassaywasper- formedusingprimerstoamplifya131-bpregionofthe16SrRNAgeneofP.acnes:forward primer5’-GCGTGAGTGACGGTAATGGGTA-3’,reverseprimer5’-TTCCGACGCGAT CAACCA-3’andTaqManprobe5’-AGCGTTGTCCGGATTTATTGGGCG-3’[24].The15-μl PCRreactionmixturecontained6,75μlofDNAsample,5pmolofeachprimerand2pmolof TaqManprobe,and1XTaqManGeneExpressionMasterMix(LifeTechnologies,USA).The QuantStudio12KFlexsystem(LifeTechnologies,USA)wasusedwiththethermalcycling PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 4/12 P.acnes'PrevalenceinHerniatedDiscs profileof50°Cfor2min,95°Cfor10minand50cyclesof95°Cfor15sand60°Cfor1min. TheP.acnesgenomeequivalentsinsampleswereestimatedwithaninternalstandardcurve preparedwithfivereplicatesofsixconcentrations(10–106copies)ofsynthesizedP.acnes amplicon(131bp)(IntegratedDNATechnologies,USA).Laboratorycontaminationcontrols describedaboveandPCRnegativecontrolswereincludedineveryPCRreaction.Assayswere doneinduplicateforeachsample,andthemeannumberofthe16SrRNAgenecopieswascal- culated.Toeliminatelaboratorycontamination,16SrRNAcountsdetectedinlaboratorycon- taminationcontrolweresubtractedfromthecopiesnumberinthetissuesamples.Thenumber ofbacterialgenomesineachsamplewasfinallycalculatedusingtheknownnumberofcopies ofthe16SrRNAoperon(3copies/cell)inP.acnes[4]andrepresentedasthenumberofbacte- rialgenomesin500ngoftotalDNAextractedfromthedisctissuesample.Humanß-globin genewasincludedasaninternalcontroltoallowassessmentofthespecimenqualityandthe nucleicacidextractionaswellastheinhibitionamplificationprocessasdescribedpreviously [24]. Dataanalysis Adescriptionofidentifiedbacterialfrequencieswasperformedandtherelationshipbetween presence/countsofP.acnesandclinicalparameterswasevaluated.Categoricalvariableswere analyzedusingatwo-sidedFisher’sexacttest,continuousvariables(genomecounts,age)with thenon-parametricMann-WhitneyUtest.Spearman’scorrelationwasusedtotesttheassocia- tionbetweenbacterialcountsreachedinthesamesamplesbydifferentmethods.Thesignifi- cancelevelwassetat0.05.ThestatisticalsoftwareusedwasPrism5(GraphPadSoftwareInc., USA). Results Patientcharacteristics Weprospectivelyenrolled290patients(171malesand119females)withanaverageageof 47±13years.Onehundredninety-twocaseswereenrolledatUniversityHospitalBrno,ninety eightcasesatSt.Anne’sUniversityHospital.Thedegenerativeintervertebraldiscsegments wereL2/L3in8(3%),L3/L4in21(7%),L4/L5in137(47%)andL5/S1in124(43%)cases.For 8patientswhounderwentadouble-leveldisksurgery,onlythecaudaldiskwasselectedto avoidastatisticalbias.Discherniationtypesincludeddiscprotrusionin23(8%),discextrusion in126(44%),anddiscsequestrationin141(48%)patients.Medicalhistoryofpreviousspinal surgerywasnotedin51(17%)cases,priorepiduralsteroidinjectionwasreceivedby14(5%) patients.Noneofthepatientsdevelopedclinicallyevidentpost-operativediscitis.Therewere nosignificantdifferencesinpatientcharacteristicsbetweenthetworecruitmentcentersregard- ingage,genderanddisease-specificclinicaldatawhichwerecollectedandusedinourstudy. Resultsofbacterialculture Bacteriawereidentifiedin130of290disctissuessamples,theother160biopsiesresultedinno bacterialcolonies.Thefollowingbacteriawereisolated:P.acnesin115cases(40%),coagulase- negativestaphylococci(CoNS)in31cases(11%)andalpha-hemolyticstreptococci(AHS)in8 cases(3%)(Fig1A).Twenty-fourpatients(8%)hadtwomicroorganismspresentinthedisc. Nopatientshadmorethantwotypesofbacteriaisolated.Weobservedsignificantvariabilityin P.acnescountsamongpositivediscsamplesrangingfrom100to9000CFU/ml(median400 CFU/ml). PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 5/12 P.acnes'PrevalenceinHerniatedDiscs PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 6/12 P.acnes'PrevalenceinHerniatedDiscs Fig1.ResultsofanaerobiccultureanddetectionofP.acnesgenomecountsindisctissuesamples.Prevalence rateofthebacteriaisolatedfromdisctissuesamples(A),stratificationofthesamplesaccordinglytobacterialcounts reachedbyculture(B)anddifferencesinthebacteriagenomecountsdetectedbyreal-timePCRingroupofpatientswith abundantP.acnesbyculture,non-abundantP.acnesandculture-negativecases(C). doi:10.1371/journal.pone.0161676.g001 Athresholdwasdefinedas(cid:1)1x103CFU/ml(75thpercentile)forthediscswithabundantP. acnes.PrevalenceofthediscsampleswithabundantP.acneswas11%(39cases);intheremain- ing29%(76cases)ofpositivediscsamplesP.acneswasnotabundant(<1x103CFU/ml). Propionibacteriumacnesgenomecountsindisctissuesamples DNAwassuccessfullyextractedfromallsamplesincludedinthestudywithconcentration rangingfrom2to45ng/μl(median13ng/μl).ThemeanCt(thresholdcycle)valueforthe internalcontrol,humanß-globingene,was24.03±1.81.Eighteencasesofthe290caseswere excludedfromstatisticalevaluationduetonegativeofß-globingene(Ct>35).ThemeanP. acnesgenomescountinthelaboratorycontaminationcontrolsampleswas4±4genomes.P. acnesgenomeswereundetectableinonly13(4%)cases.ThenumberofP.acnesgenomesin the259P.acnes-positivedisctissuesrangedfrom2to5831withamedianof260genomesper 500ngoftotalDNA.ThereweresignificantdifferencesinthenumberofP.acnesgenomes detectedinthesampleswithabundantP.acnesbyculture(1039±244genomes),whencom- paredtosampleswithnon-abundantP.acnes(448±98genomes)andsamplesnegativebycul- ture(415±57genomes)(forbothP<0.0001,Fig1C).WealsofoundsignificantPearson correlationbetweenCFU/mlandP.acnesgenomecountsdetectedbyreal-timePCRinpatients positivebyculture(r=0.4363,p<0.0001).TherewasnodifferenceinthenumberofP.acnes genomesbetweendisctissuesampleswithnon-abundantP.acnesandsamplesnegativebycul- ture(p=0.6973). RelationshipsofPropionibacteriumacnesandpatientcharacteristics TheaverageageofpatientshavingdiscswithabundantP.acnesbyculturewassignificantly lower(42versus48years;p=0.0086).Therewerenosignificantdifferenceswhencomparing thegroupsofpatients(i.e.,abundantP.acnes,non-abundantP.acnes,ornegativecultures)in gender,prevalenceofpreviousspinalsurgery,prevalenceofpriorepiduralsteroidinjection, distributionofherniationtype,oraffectedintervertebrallevel(summarizedinTable1).With theexceptionoftheage,therewerenosignificantassociationsfoundbetweenP.acnespreva- lenceandclinicalcharacteristicsincludingthesituationinwhichallpatientswithapositive culture(abundant+non-abundant)wereconsideredpositiveforstatisticalevaluationortheP. acnesgenomecountswerecomparedbetweengroups(allp>0.05). Discussion Traditionally,mechanical,degenerative(age-related),traumaticandgenetics-basedtheories havebeenproposedaspossibleetiologiesofdegenerativediscdisease[25],butevidencehas emergedoverthelastdecadeshowingthatlow-gradeinfections,mostlybyP.acnes,playinga potentialcausativeroleindiscdegenerationandresultantdisc-herniationandradicularpain [11,19].However,thepotentialrelationshipbetweenintervertebraldiscdegenerationand chronicinfectionbylow-virulenceP.acnesremainscontroversial,withcontradictoryevidence intheliterature.WesuggestthatforaccuratedetectionofP.acnes,itiscriticaltoanticipateits existenceinitsbiofilmform[5,26,27]andtousequantitativemethodstodeterminebacteria counts.Unfortunately,thisapproachhasnotbeenutilizedinanyofthepublishedstudiesin thisfield.Inthecurrentstudy,wehomogenizeddiscsamplestodisruptbiofilmaggregates PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 7/12 P.acnes'PrevalenceinHerniatedDiscs Table1. RelationshipsbetweenstrongpositivityofP.acnesinthediscandepidemiological/clinicalcharacteristicsofthepatients. Parameters AbundantP.acnesbycultureN(%) Non-abundantP.acnesornegativecultureN(%) P-value Gender Male 28(16%) 144(84%) 0.1144 Female 11(9%) 108(91%) Age Mean±SD 42±12y 48±13y 0.0086 Previousspinalsurgery Yes 8(16%) 43(84%) 0.5019 No 30(14%) 209(86%) Priorepiduralinjection Yes 3(21%) 11(79%) 0.4128 No 111(40%) 165(60%) Typeofherniation Protrusion 3(13%) 20(87%) 0.6445 Extrusion 14(11%) 112(89%) Sequestration 21(15%) 119(85%) Intervertebrallevel L2/L3 1(13%) 7(87%) 0.6313 L3/L4 1(5%) 20(95%) L4/L5 15(16%) 81(84%) L5/S1 23(14%) 142(86%) CoNS,coagulase-negativestaphylococci. doi:10.1371/journal.pone.0161676.t001 (whichifundisruptedoftenleadtonegativecultureresults[27])toeliminatefalsenegativity, andusedquantitativeanaerobiccultureandreal-timePCRtodeterminebacterialcounts/ genomesasoneofthecriteriatoeliminatepotentialcontaminationandfalsepositivity. Weprospectivelyenrolled290patientsundergoingmicrodiscectomyforlumbardischerni- ation,whichisthelargestseriesofpatientstodate,andexaminedtheirintraoperativedisc biopsiesbyquantitativecultureandreal-timePCR.Weisolatedthreebacterialspeciesbycul- ture:P.acnes,CoNSandAHSin40%,11%and3%ofcases,respectively.Ourdataareinagree- mentwithamajorityofthepreviousreportsdescribingP.acnesandCoNSasthemost frequentlyisolatedbyanaerobicculture[12,14–17].OveralltheP.acnespositivityrate observedinourstudyissimilartotheresultsofStirlingetal.[12],Arndtetal.[16]andAlbert etal.[17],whoobserved44%,35%and40%positivityrate,respectively.Analogicallytoour results,5%,14%and31%prevalenceofCoNSwasdescribedinthreeothersstudies[12,14,16]. Weusedstandardsurgicalcareprotocols,includingtheuseofprophylacticperioperative antibiotics(cefazolin),thusensuringpatientsafetywhileconductingourresearch.Werea- sonedthatcephalosporinprophylacticantibioticswouldnotaffecttheresearchresultsbecause theseantibioticsdonotpenetrateintotheintervertebraldiscsandbecauseP.acnesbiofilm withinthediscisantibioticresistantatthetypicallyuseddoses[28].Intwoprotocols,prophy- lacticantibioticswereadministeredaftercollectionofthebiopsiestoavoidinhibitionofany bacteriainthesample[17],orwerenotadministeredatall[22].Inthefirstcase,thepositivity rateofP.acneswasidenticalwithourstudy(40%inboth),inthesecondstudyP.acnespositiv- itywasonly4%,indicatingthatprophylacticcefazolinedoesnothaveanyinhibitoryeffectson theP.acneswithinthedisc. NoneofthepreviousstudiesdeterminedP.acnescountsinthediscsanddistributionofthe bacteriacountswithintheircaseseries.WedescribedtherangeofP.acnescountsobtainedby PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 8/12 P.acnes'PrevalenceinHerniatedDiscs cultureandobservedan11%prevalenceofintervertebraldiscswithabundantP.acnes ((cid:1)1x103CFU/ml).Wesuggest,thatthisquantity-adjustedprevalenceislessbiasedbycon- taminationthanoverallpositivity.SimilarprevalenceoftheP.acnespositivediscsampleswere observedbyAgarwaletal.[15],Cosciaetal.[14]andZhouetal.[18]describing13%,19%and 24%positivityrate,respectively.Asquantitativedatafromotherstudiesarenotavailable,and differencesinthepositivityratesdiffersignificantly(from4to44%),itislikelythatsome authorsevaluatedweakpositivityascontaminationandothersaspositivity. However,therearealsostudiesdescribingloworzeroP.acnespositivityofdiscsintheir caseseries[21–23].Forinstance,P.acneswasnotisolatedfromanyof30discsamplesinthe studybyBen-Galimetal.[21],whoimplementedinoculationofculturesdirectlyintheoperat- ingtheatretominimizetheriskofcontamination.Authorsofthisstudysuggestthatthehigh prevalenceofP.acnesobservedinotherstudiesmainlyreflectscontamination.Wespeculate thatthisunusualapproachdidnotprovideforsufficienthomogenizationofthetissueanddis- ruptionofP.acnesbiofilms,whichcombinedaccountsfortheirnegativecultureresults.Simi- larly,inthelarge-scalestudyonpatientswithchroniclowerbackpain,discfragmentswere cultureddirectlywithouttissueprocessingorhomogenization,andP.acneswereisolatedin only2of313cases[23,29]. Weimplementedareal-timePCRassayandlaboratorycontaminationcontrolstoaccu- ratelyquantifyP.acnesgenomesdirectlyinthedisctissuesamples.ThenumbersofP.acnes genomesinthediscs,whichwereP.acnesabundantbyculture,weresignificantlyhigherwhen comparedtonon-abundantorP.acnesnegativediscs.Therewasnodifferenceinthenumbers ofP.acnesgenomesbetweenthediscswithnon-abundantP.acnesandnegativesamplesby culture,supportingapotentialcontaminationoriginofthediscsampleswithnon-abundantP. acnesandaccuracyoftheempiricalthreshold((cid:1)1x103CFU/ml)forthesampleswithabun- dantP.acnes.Onlyin13(4%)cases,werenoP.acnesgenomesdetected.Thisisinagreement withoutputsoflarge-scalestudiesbasedonnext-generationsequencingofP.acnesDNAina varietyofclinicalspecimensconcludingthatwhenhighlysensitivemolecularmethodsare employed,P.acnesDNAcouldbedetectedinpracticallyallsampletypes[30].Moreover,it wasshownthatP.acnesDNAisafrequentcontaminantofcommercialTaqpolymerasesand PCRsolutions[31],highlightingthenecessityofquantitativeinformationtodistinguish betweencontaminationandpositivity[32].Untilnow,onlyoneteamfocusedondirectdetec- tionofP.acnesDNAindisctissuebyqualitativeend-pointPCR[17].OthersusedPCRonly forverificationofP.acnesDNAinpurifiedcolonies[18].Albertetal.observedconsistent resultsofcultureandPCRmethods;and,surprisingly,thecasesnegativebyculture(60%)were negativebyPCR[17],whichcouldbeexplainedbythedecreasednumberofcycles(only35)in theirassay,probablytoartificiallydecreasethesensitivityoftheirmethod. WedidnotobserveanysignificantassociationbetweenP.acnespositivityandprevalenceof previousspinalsurgeryandpriorepiduralsteroidinjectionindicatingendogenousoriginofP. acnesandtheirroleindegenerativediscdiseasemorethantheiriatrogenicoriginthroughdisc contaminationinthepreviousspinalsurgeries.P.acnespositivityrateswereindependentof gender,typeofherniation,andaffectedspinalsegment.Theaverageageofpatientshaving discswithabundantP.acneswerelower(42versus48years).Wehypothesize,thatP.acnes infectioncouldaccelerateregularmechanical,age-related,degenerativeprocessinaffected individualsandresultinthenecessityofearliersurgicalintervention. Alsoofnoteisthetwomostcommoncommensals,P.acnesandcoagulase-negativestaphy- lococci,werealsothetwomostcommonbacteriafoundinthedisctissuesamples,which reflectsthecompellingneedtogainanabilitytodiscriminatebetweenacontaminationandan infection. PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 9/12 P.acnes'PrevalenceinHerniatedDiscs Thisstudyhasseverallimitations.Aerobiccultureswerenotperformedgivendisctissue originatesinanotablyanaerobicenvironment.Asweconsidertissuehomogenizationacritical stepoftheexperimentalprotocol,morestandardizedhomogenizationmethodsthanmortar andpestleshouldbeimplemented.WeassumethatthebiofilmformofP.acnesistypically presentwithinthedisc,butdonotprovidedirectevidenceofP.acnesbiofilmsfromthedisctis- suebymicroscopicmethods.However,inthefieldoforthopedicinfections,thereisstrongevi- denceofP.acnesformingabiofilm[26,27].Asdisctissuefromage-matchedhealthy individualsisnotavailable,theidentificationofP.acnesinbiopsiesfromcomparablehealthy individualscannotberuledout.Further,thelackofcontrolculturescannotexcludethepossi- bilityofcontaminationfromthelaboratory,operatingroom,surgicalfield,orskin.With exceptionofone[22],mostofthepreviousstudiesthatincludednegativecontrolsprovedthat theyarelargelysterile[12,14,18].Sincepositiveendogenouscontrolsdonotnecessarilycon- notecontaminationofthediscsample,wedonotbelievethatendogenouscontrolsaretheopti- malsolutiontoidentifycontaminateddiscsamples.Inourstudy,P.acnescountsandthe numberofP.acnesgenomeswereimplementedasoneofthecriteriatoeliminatepotential contamination.ThefinalanswerwithregardtodistinguishingendogenousP.acnesinfection ofthediscfromskincontaminationwillprobablyutilizecomparativegenomicstodifferentiate P.acnesgenomesfromtheskinanddisctissuefromagivenindividual[33,34]. Inconclusion,toourknowledgethisisthefirststudythatprovidesquantitativeinformation aboutP.acnesindisctissuesamplesinthelargestseriesofpatientswithlumbardischernia- tion–wedemonstratedan11%prevalenceofthedischerniationsampleswithanabundanceof P.acnes.Because“findingabundantmicroorganisminorganismssufferingfromthedisease”is oneofthemostimportantofKoch’spostulates,injudgingtherelationshipbetweenaspecific microbeandaspecificdisease,webelievethatourfindingssupportthetheorythatP.acnesis involvedinthepathogenesisofatleastasubsetofpatientswithdegenerativediscdisease. FuturestudiesareneededtoevaluaterelationshipbetweenP.acnesinfectionandclinicalout- comesofthesepatients. AuthorContributions Conceptualization:MNCFRRJJESMSK.MavrommatisFSAJLSCBVAFOS. Datacuration:MNCFSAOSTMJSCB. Formalanalysis:MNCOS. Investigation:FRFSATMEMJSMH. Methodology:MNCFRRJJESMSK.MavrommatisFSAJLSCBVAFOS. Projectadministration:MNCOSFRCBRJ. Resources:FROSRJRLMSK.Maca. Supervision:VAF. Visualization:MNCOSJCBFSA. Writing-originaldraft:MNCFSAOSJCB. Writing-review&editing:MNCFRTMRJMSJESMHJSEMJCBFSAK.MacaRLTAMC JLSTWGDEZLGK.MavrommatisVAFCBOS. PLOSONE|DOI:10.1371/journal.pone.0161676 August18,2016 10/12

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4 [email protected] (OS); [email protected] (MNC). Abstract. Background. The relationship between intervertebral disc degeneration and chronic infection by Propio- nibacterium acnes is controversial with contradictory evidence available in the literature. Previous studies
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