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HOLOTYPEHLA™96/5A&B
USERMANUAL
FORRESEARCHUSEONLY
V2.1
OmixonLimited
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TableofContentsDOCUMENTHISTORY...........................................................................................................................................4THEPRINCIPLEOFTHEMETHOD:NGS-BASEDHLATYPINGFORTHEILLUMINAMISEQ.........................................6HOLOTYPEHLAPACKINGLIST...............................................................................................................................7
PRIMERCOMPONENTBOX..............................................................................................................................................7LIBRARYPREPARATIONREAGENTSCOMPONENTBOX...........................................................................................................796-WELLADAPTORPLATE...............................................................................................................................................7EXCELWORKBOOK........................................................................................................................................................7SOFTWARE–OMIXONHLATWIN....................................................................................................................................7
RECOMMENDATIONS...........................................................................................................................................8DNAEXTRACTIONRECOMMENDATIONS............................................................................................................................8TECHNICALANDEQUIPMENTRECOMMENDATIONS..............................................................................................................8ASSOCIATEDREAGENTRECOMMENDATIONS.......................................................................................................................8
MiSeqReagentKitcapacity.................................................................................................................................9RECOMMENDEDSUPPLIES...............................................................................................................................................9
LEGALNOTICE....................................................................................................................................................11SUMMARYOFSTEPS..........................................................................................................................................12GLOSSARY/DEFINITIONS.....................................................................................................................................13STEP0–GENOMICDNAPREPARATION..............................................................................................................14STEP1–HLAAMPLIFICATIONMASTERMIXPREPARATION................................................................................15
REAGENTLIST.............................................................................................................................................................15PROTOCOL.................................................................................................................................................................15
MasterMix:HLA-A,B,CandDRB1....................................................................................................................15MasterMix:HLA-DQB1Set3.............................................................................................................................16
STEP2–HLACLASSIANDIIAMPLIFICATION......................................................................................................17REAGENTLIST.............................................................................................................................................................17PROTOCOL.................................................................................................................................................................17
TaqPolymerase-LoadedMasterMix:HLA-DQB1Set3......................................................................................17ClassIAmplification(HLA-A,BandC)...............................................................................................................18ClassIIAmplification(HLA-DRB1andDQB1).....................................................................................................18ExpectedAmpliconSizes....................................................................................................................................18
STEP3–AMPLICONQUANTITATIONANDNORMALIZATION(USINGAPLATEFLUOROMETER)...........................19REAGENTLIST.............................................................................................................................................................19PROTOCOL.................................................................................................................................................................19
Ampliconpooling...............................................................................................................................................20ExoSAP-ITExpressPCRPurification....................................................................................................................21
STEP4–LIBRARYPREPARATION........................................................................................................................22REAGENTLIST.............................................................................................................................................................22PROTOCOL.................................................................................................................................................................22
FragmentationMasterMix................................................................................................................................22FragmentationProgram....................................................................................................................................23EndRepairMasterMix......................................................................................................................................24
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EndRepairProgram...........................................................................................................................................24LigationMasterMix...........................................................................................................................................25LigationProgram...............................................................................................................................................25Poolingandlibrarypurification.........................................................................................................................26
STEP5–LIBRARYSIZESELECTION.......................................................................................................................28REAGENTLIST.............................................................................................................................................................28PROTOCOL.................................................................................................................................................................28
STEP6–LIBRARYQUANTIFICATIONUSINGANINTERCALATINGDSDNAFLUORESCENTDYE...............................29REAGENTLIST.............................................................................................................................................................29PROTOCOL.................................................................................................................................................................29
STEP7–SEQUENCINGONILLUMINAMISEQ......................................................................................................31REAGENTLIST.............................................................................................................................................................31
MiSeqReagentKitcapacity...............................................................................................................................31PROTOCOL.................................................................................................................................................................31
STEP8–ANALYSISOFHLASEQUENCINGDATA..................................................................................................33AUTOMATEDPROTOCOL...............................................................................................................................................33
ITSetupandConfiguration................................................................................................................................33ProtocolperAnalysis.........................................................................................................................................33
MANUALSERVERPROTOCOL.........................................................................................................................................33ITSetupandConfiguration................................................................................................................................33ProtocolperAnalysis.........................................................................................................................................33
MANUALDESKTOPPROTOCOL.......................................................................................................................................33ITSetupandConfiguration................................................................................................................................33ProtocolperAnalysis.........................................................................................................................................34
TECHNICALASSISTANCE.....................................................................................................................................35PhoneSupport:..................................................................................................................................................35
SUPPLEMENTALFIGURES....................................................................................................................................36PLATEEXAMPLEFORAMPLICONPLATE,AMPLIFICATIONPLATE,DILUTIONPLATE,AMPLICONQUANTITATIONPLATE(FORANINDIVIDUALLOCUS)&REACTIONPLATE...........................................................................................................................36STANDARDSQUANTITATIONPLATEEXAMPLE....................................................................................................................37KAPALIBRARYQUANTITATIONQPCRPLATEEXAMPLE......................................................................................................37
APPENDIX1:PIPPINPREP...................................................................................................................................38PROGRAMMINGTHEPIPPINPREP...................................................................................................................................38RUNNINGTHEPIPPINPREP...........................................................................................................................................38
APPENDIX2:AMPLICONQUANTITATIONUSINGAQPCRINSTRUMENT..............................................................41REAGENTLIST.............................................................................................................................................................41PROTOCOL.................................................................................................................................................................41
APPENDIX3:LIBRARYQUANTITATIONUSINGAQPCRINSTRUMENT..................................................................43REAGENTLIST.............................................................................................................................................................43PROTOCOL.................................................................................................................................................................43
qPCRPrimerMix................................................................................................................................................43qPCRMasterMix...............................................................................................................................................44
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DocumentHistoryVersion Date DescriptionofChanges ApprovalName1.5 January,2015 InitialVersion PeterMeintjes1.6 March,2015 DQB Enhancer combination, general edits,
Appendix2:SampleSheetPeterMeintjes
1.7 June,2015 ExoSAP-IT Step Change, DQB1 Set 1&2pooling, DQB1 Set 1 optional, <16samples/run,PippinPrep0.8
PeterMeintjes
1.7.1 June,2015 DPB1 caps changed from Clear to Purple,DQA1 caps changed from Clear to Brown.MiSeq Reagent Nano Kit v2 requirementsupdated.
PeterMeintjes
1.7.2 July,2015 MiSeq Reagent Kit v2 and MiSeq ReagentNanoKitv2requirementsupdated.
PeterMeintjes
1.7.3 November,2015 Amplification verification and quantitationmay be optional after sufficient andconsistentexperience.
PeterMeintjes
1.7.4 February,2016 IncreasedvolumeofEnhancer2,Enhancer2should now be saved after Combined DQBEnhancerismade,addednewDRB4MasterMixformulation,increasedthevolumeusedin Fragmentation and End Repair mastermixforfullplate,androundedsomevaluestothenearesttenth.
EfiMelista
1.7.5 April,2016 Changedwordingfrom“LR-PCRenzyme”to“Taq Polymerase” based on Qiagen’sdocumentation change. Removed X2 fromHolotype HLA product configuration name.Approval name has been added ondocumenthistory.
EfiMelista
1.7.6 April,2016 DQB1set1andset2statementupdate EfiMelista1.7.7 July,2016 Updated library preparation reagent
volumes,additionofadaptorplateA2andBinformation.
EfiMelista
2.0 January,2016 “DQB” removal from the DQB Enhancers,Gel verification after LR-PCR is optional,amplicon quantitation simplification, per-sample pooling volume change in 11-locuskits, ExoSAP-IT replacement by ExoSAP-ITExpress,Qubituseforlibraryquantitation.
EfiMelista
2.1 September,2016 DQB1set1andset2primermixreplacedbyDQB1 set 3, library quantitation methodwording update, end repair reaction timedecrease, ligation reaction time decrease,SamplesheetremovedfromAppendices
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ThePrincipleoftheMethod:NGS-basedHLAtypingfortheIlluminaMiSeqFormany years theHLA community has beenworking toward amethod thatwill accuratelyidentifytheextensivepolymorphismoftheHLAgenesandoftheirgeneproducts.TheadventofPCR,combinedwithothertechnologies(Sangersequencing,SSOP,SSP,Luminex),providedaformula for significantly improving the detection of HLA polymorphisms albeit with severallimitationsthatcontinuetoinhibitourabilitytocomprehensivelycharacterizetheHLAgenes.Technologies developed over the last several years, cumulatively called Next GenerationSequencing (NGS),haveprovidednewopportunities thatallowthecompletecharacterizationoftheHLAgenesinhaploidfashion.NGShastwodistinctfeatures,1)clonalsequencingofDNAfragments, and 2) tremendously high throughput. NGS provides the capability to phasepolymorphismstherebyeliminatingallambiguitiesandprovidesHLAtypingatthethreetofourfieldlevelwithoutreflexivetesting,therebyintroducingapotentiallytotalsolutiontotheHLAtypingproblem.Theprotocoldescribedheretakesadvantageofthistechnologyandcombineslong-range PCR amplification of HLA geneswith sequencing on the IlluminaMiSeq platform.MorespecificallytheHLAgenesA,B,CandDQB1areamplifiedfortheirentirecodinglength,includingelementsofthe5’and3’untranslatedregions,whileDRB1isamplifiedfromintron1tointron4.Theampliconsarethenprocessedthroughaseriesofstepsthat:1. FragmenttheampliconstoasizeappropriateforsequencingontheIlluminaplatform,
2. Blunt-endandadenylatetheendsofthefragmentedampliconsand
3. LigateadaptorsequencesthatareusedthroughouttheprocessontheMiSeqtocapture,amplify, and sequence the DNA. The adaptors also include an index which is a shortsequence, unique to each adaptor, which identifies the origins of the library(sample/locus).
Afterpoolingtheindexedlibraries,sizeselectionandquantitation,thesampleisloadedontheMiSeqforsequencing.Thewholeprocesstakes3-5daysdependingontheselectionoftheflowcellontheIlluminaplatform.ThegenerateddataareanalyzedusingtwodifferentalgorithmsinHLATwin™(www.omixon.com).TheuseoftwoindependentalgorithmsinHLATwinprovidesthehighestlevelofconfidencesothattheHLAgenotypingresultscanbereportedimmediatelywithoutfurtherattention.Sampleswithquestionableorambiguousgenotypingsareflaggedbythesoftwaretobeanalyzedmanually.
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HolotypeHLAPackingList
PrimerComponentBoxPrimermix Rxns Vol/tube #Tubes ColorcodeHLA-A 96 220μL 1 YellowHLA-B 96 220μL 1 RedHLA-C 96 220μL 1 OrangeHLA-DRB1 96 220μL 1 GreenHLA-DQB1(Set3) 96 220μL 1 BlueEnhancer1 96 1100μL 1 ClearEnhancer2 96 300μL 1 Clear
LibraryPreparationReagentsComponentBoxReagent Rxns Vol/tube #Tubes ColorcodeFragmentationEnzyme(A) 96 278μL 1 YellowFragmentationBuffer(B) 96 278μL 1 RedEndRepairEnzyme(C) 96 162μL 1 GreenEndRepairBuffer(D) 96 324μL 1 OrangeLigationEnzyme(E) 96 324μL 1 BlueLigationBuffer(F) 96 1800μL 2 Black
96-wellAdaptorPlateIndexedadaptorsina5μLsolutionforgenerating96individualsequencinglibraries.Two (2) Adaptor Plate configurations are available containing 96 individual indices. Adaptorplates, that contain96 indicesonly areavailable in the following configurations:A (i1-i96),B(i97-i192).
ExcelWorkbookAnExcelWorkbookisprovidedtosupporttheHolotypeHLAprotocolwithvolumecalculations,platelayouts,reagenttraceability,recordkeepingandMiSeqSampleSheetgenerationofallofthe supported adaptor plate configurations (A, B). If youdonot have a copy, please [email protected].
Software–OmixonHLATwinContact [email protected] for Omixon HLA Twin license associated with your purchase ofHolotypeHLA.
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Recommendations
DNAExtractionRecommendations§ HighqualitygenomicDNA(gDNA)extractedfromwholeblood,bloodcells(B-celllines,
buffycoats,cordbloodoranyfractionofwhitebloodcells),salivaandbuccalswabscanbeused.FortheamplificationofHLA-A,HLA-B,HLA-C,HLA-DRB1andHLA-DQB10.5–0.75µgofgDNAisrequired.
TechnicalandEquipmentRecommendations§ Thermalcyclerwith96-wellformat§ Platefluorometer(oranyinstrumentcapableoffluorescencedetectionin96-wellplate
format,forusewiththePromegaQuantiFluordsDNASystem)§ PippinPrep(Cat#PIP0001)orBluePippin(Cat#BLU0001)bySAGEScience§ Qubitfluorometer(Cat#Q33216,ThermoFisherScientific)§ qPCRinstrumentwith96or384-wellplateformat(optional)§ IlluminaMiSeq(Cat#SY-410-1003)§ 64-bitcomputerwithminimum4Coresand16GBofRAM§ Long-termdatastorage(approximately2TBofdataperMiSeqperyear)
AssociatedReagentRecommendations§ LongRangePCRkitsfromQiagen(Cat#206401,206402or206403)
§ Eachsamplerequires2.4μLofTaqPolymerase§ Cat#206401LongRangePCRkit(20)contains8μLofTaqPolymerase§ Cat#206402LongRangePCRkit(100)contains40μLofTaqPolymerase§ Cat#206403LongRangePCRkit(250)contains100μLofTaqPolymerase
§ ExoSAP-IT Express from Affymetrix (Cat#75001-200, 75001-1ML, 75001-4X-1ML or75001-10ML)
§ Eachpooledsamplerequires4μLofExoSAP-ITExpressenzyme§ Cat#75001-200contains200μLofExoSAP-ITExpressenzyme§ Cat#75001-1-MLcontains1mLofExoSAP-ITExpressenzyme§ Cat#75001-4X-1MLcontains4mLofExoSAP-ITExpressenzyme§ Cat#75001-10MLcontains10mLofExoSAP-ITExpressenzyme
§ QubitdsDNABRAssayKit(Cat#Q32850orQ32853)§ Cat#Q32850for100assays§ Cat#Q32853for500assays
§ Library Quantification Kit – Illumina/Universal from KAPA Biosystems (Cat# KK4824)(optionalifusingaqPCRinstrument)
§ QuantiFluordsDNASystemfromPromega(Cat#E2670)§ AgencourtAMPureXPbeadsfromBeckmanCoulter(Cat#A63880,A63881,orA63882)
§ EachHolotypeHLArunrequiresamaximumof900μLofAMpureXPbeads
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§ Cat#A63880contains5mLofAMPureXPbeads§ Cat#A63881contains60mLofAMPureXPbeads§ Cat#A63882contains450mLofAMPureXPbeads
§ Gelcassette,1.5%agarose,dyefreewithinternalstandard(MarkerK/R2),forthePippinPrep/BluePippin(Cat#CDF1510forPippinPrepandBDF1510forBluePippin)
§ Moleculargradeethanol(AnhydrousAlcohol)§ Moleculargradewater(DNaseandRNasefree)§ Sodiumhydroxide§ 1×TEbuffer(pH8.0)§ MiSeqReagentKitfromIllumina
MiSeqReagentKitcapacityIlluminaMiSeqReagentKit
TimeHours
24/7Samples
24/11Samples
96/5Samples
96/7Samples
96/11Samples
Std300Cycle(MS-102-2002)
~24 24 24 96 96 72
Micro300Cycle(MS-103-1002)
~19 24 20 40 28 20
Nano300Cycle(MS-103-1001)
~17 6 4 8 6 4
Std500Cycle(MS-102-2003)
~39 24 24 96 96 96
Nano500Cycle(MS-103-1003)
~28 12 8 16 12 8
RecommendedSupplies§ 1.5mLmicrocentrifugetubes§ 1.5mLlow-bindmicrocentrifugetubes§ 2.0mLlow-bindmicrocentrifugetubes(EppendorfDNALoBindCat#022431048
recommended)§ 0.5mlthinwalltubesforQubitinstrument(QubitAssaytubesCat#Q32856
recommended)§ Adjustablevolumepipettes(1.0–1000μLcapacity)§ 8-channeladjustablevolumepipettes(1.0-100μLcapacity)§ 96-wellplatescompatiblewiththethermalcycler§ 96-wellopticalplatescompatiblewiththeplatefluorometer§ 96-wellplatescompatiblewiththeqPCRinstrument(optional)§ Platesealsforgeneraluse§ Platesealscompatiblewiththethermalcyclers(testedforlongrangePCR)§ OpticalplatesealscompatiblewiththeqPCRinstrument(optional)§ Magneticstandcompatiblewith2mLmicrocentrifugetubes§ 96-wellcoolerracks(2pieces)
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§ 50mLconicaltubes§ 50mLreservoirs
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LegalNoticeThe Holotype HLA User Manual and all contents are proprietary to Omixon Biocomputing("Omixon"), and are intended solely for the contractual useby its customer in regard to theproduct(s)describedhereinandfornootherpurpose.Thisdocumentanditscontentsshallnotbe used or distributed for any other purpose and/or otherwise communicated, disclosed, orreproducedinanywaywhatsoeverwithoutthepriorwrittenconsentofOmixon.Omixondoesnotconveyanylicenseunderitspatent,trademark,copyright,orcommon-lawrightsnorsimilarrightsofanythirdpartiesbythisdocument.UseofOmixonHolotypeorMonotypeHLA(includingsoftwareandassay)isgovernedbyTermsandConditionsGoverningOmixonProducts(www.omixon.com/supply-agreement/),whichreferencestheOmixonHLATwinEULA(www.omixon.com/hla-twin-eula/).
UseofOmixonTargetsoftwareisgovernedbytheOmixonTargetEULA(www.omixon.com/omixon-target-eula/).
UseofOmixonHLATwinsoftwarealoneisgovernedbytheOmixonHLATwinEULA(www.omixon.com/hla-twin-eula/).
UseofOmixonHLAExploresoftwareisgovernedbytheOmixonHLAExploreEULA(www.omixon.com/hla-explore-eula/).
The instructions in this document must be strictly and explicitly followed by qualified andproperly trained personnel in order to ensure the proper and safe use of the product(s)describedherein.Allofthecontentsofthisdocumentmustbefullyreadandunderstoodpriortousingsuchproduct(s).FAILURE TO COMPLETELY READ AND EXPLICITLY FOLLOW ALL OF THE INSTRUCTIONSCONTAINED HEREIN MAY RESULT IN DAMAGE TO THE PRODUCT(S), INJURY TO PERSONS,INCLUDINGTOUSERSOROTHERS,ANDDAMAGETOOTHERPROPERTY.OMIXON DOES NOT ASSUME ANY LIABILITY ARISING OUT OF THE IMPROPER USE OF THEPRODUCT(S)DESCRIBEDHEREIN(INCLUDINGPARTSTHEREOFORSOFTWARE)ORANYUSEOFSUCHPRODUCT(S)OUTSIDETHESCOPEOFTHEEXPRESSWRITTENLICENSESORPERMISSIONSGRANTED BY OMIXON IN CONNECTION WITH CUSTOMER'S ACQUISITION OF SUCHPRODUCT(S).FORRESEARCHUSEONLY©2017OmixonBiocomputingLtd.Allrightsreserved.
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SummaryofSteps
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Glossary/Definitions§ AmpliconPlate–AlternativenameforanAmplificationPlate§ AmpliconQuantitationPlate–96-wellplate compatiblewith theplate fluorometeror
qPCRmachinewheretheampliconsarequantitated.§ AmplificationPlate–96-wellPCRplateusedtoamplifytheHLAloci.§ Final Library – Library that includes all Sample Libraries ready to be sequenced in a
singleMiSeqrun.§ Reaction Plate – Platewhere the sequential reactions that fragment, end repair, and
ligatetheindexedadaptorstotheSampleLibrariesareperformed.§ ReagentPlate–PlateusedtoaliquotthevariousreagentsusedtopreparetheLibraries§ Sample Library – A library prepared by combining (pooling) all HLA loci for a given
sample.§ PooledAmpliconsPlate:Platecontainingasamplelibrary(alllocicombined)perwell.§ StandardsQuantitationPlate–96-wellplatecompatiblewiththeplatefluorometeror
qPCRmachinewhereDNAstandardsareplacedtoallowforampliconquantitation.
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Step0–GenomicDNAPreparationDuration:~1hour45minutesIsolategDNAfromwholeblood,bloodcells(B-celllines,buffycoats,cordbloodoranyfractionofwhitebloodcells),salivaandbuccalswabs.gDNAshouldbedissolvedinwaterastheEDTAinTE buffer can inhibit long-range PCR reactions and its recommended concentration is 20-30ng/ul.Wehighlyrecommendtouseafluorescence-basedquantitationmethodtodeterminethegDNAconcentration.Itsquality,asevaluatedbyspectrophotometry,shouldbe:
1. A260nm/280nmabsorbanceratiobetween1.7and1.9.2. A260nm/230nmabsorbanceratioof1.7orgreater.3. Minimal degradation. DNA that is old or has gone through repeated
freeze/thawswillsufferfrommoredegradation.FortheamplificationofHLA-A,HLA-B,HLA-C,HLA-DRB1andHLA-DQB1,0.5–0.75µgofgDNAisrequiredforeachsample.
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Step1–HLAAmplificationMasterMixPreparationDuration:~1hour50minutesThepurposeofthisstepistopreparelocus-specificMasterMixestoamplifyeachtargetedHLAlocus individually.The lociamplifiedbythisprotocolareHLA-A,HLA-B,HLA-C,HLA-DRB1andHLA-DQB1.Note: TheMasterMixes prepared in this step include all reagents needed for amplificationexcepttheTaqPolymerase.
ReagentlistItem Storage SuppliedbyHLA-APrimerMix -20°C OmixonHLA-BPrimerMix -20°C OmixonHLA-CPrimerMix -20°C OmixonHLA-DRB1PrimerMix -20°C OmixonHLA-DQB1(Set3)PrimerMix -20°C OmixonEnhancer1 -20°C OmixonEnhancer2 -20°C OmixonLongRangePCRBuffer(10×) -20°C QiagendNTPs(10mMeach) -20°C QiagenMoleculargradeH2O -20°C Qiagen
Protocol
1.1 - Removeall primermixes, Enhancer 1 and2, thedNTPs and the Long-RangePCRBuffer(10×),fromstorageandthawatroomtemperature.
1.2 - Prepare the Combined Enhancer: add 132 μL of Enhancer 2 into the Enhancer 1 tube.RelabelEnhancer1tubeasCombinedEnhancer.
1.3 -PrepareaMasterMixforeachPrimerMixaccordingtothetablesbelow:
MasterMix:HLA-A,B,CandDRB1
Reagent Volume/sample/locus Volume/96samples/locusPrimerMix 2μL 204μLLongRangePCRBuffer(10×) 2.5μL 255μLdNTPMix(10mMeach) 1.25μL 127.5μLMoleculargradeH2O 13.85μL 1412.7μLTotalVolume 19.6μL 1999.2μL
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MasterMix:HLA-DQB1Set3Reagent Volume/sample/locus Volume/96samples/locusPrimerMix 2μL 204μLLongRangePCRBuffer(10×) 2.5μL 255μLdNTPMix(10mMeach) 1.25μL 127.5μLCombinedEnhancer 5.6μL 571.2μLMoleculargradeH2O 7.85μL 800.7μLTotalVolume 19.2μL 1958.4 μL1.4 –VortexeachMasterMixandspinitdownfor1second.PlaceMasterMixesonice.
1.5 -DiluteallgDNAstoaconcentrationof30ng/μL(minimumvolumeis35μL).
Note: Holotype HLA includes sufficient reagents for 96 reactions plus additionalvolumeforpipettinglossandfailedamplification.
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Step2–HLAClassIandIIAmplificationDuration:~7hours10minutesThepurposeof Step2 is to amplify theHLA loci.HLAClass I andClass II amplificationshavebeen optimized using two separate sets of PCR conditions. Once the PCR reactions arecompleted,amplificationisverifiedbyagarosegelelectrophoresis(optional).
Quicktip–Theagarosegelelectrophoresis(step2.5),whilerecommended, isnotrequiredtosuccessfullycompletetheHolotypeHLAprotocol.Whenampliconsarequantitated(Step3),anyconcentrationabove50ng/μL isconsideredasuccessfulamplification.Agarosegelelectrophoresis isanimportantqualitycontrolstepandshould not be skippedwithout sufficient experiencewith the completeHolotypeHLAprotocol.
ReagentlistItem Storage SuppliedbyHLA-AMasterMix -20°C Step1HLA-BMasterMix -20°C Step1HLA-CMasterMix -20°C Step1HLA-DRB1MasterMix -20°C Step1HLA-DQB1(Set3)MasterMix -20°C Step1TaqPolymerase -20°C QiagengDNA 4°C UserMoleculargradeH2O 20°C User
Protocol2.1–RemovetheTaqPolymerasefromstorage,spin itdown,andadd it toeachMasterMixaccordingtothetablesbelow,rinsingthepipettetipsthoroughlybypipetting:
TaqPolymerase-LoadedMasterMix:HLA-A,B,CandDRB1Reagent Volume/sample/locus Volume/96samples/locusMasterMixfromStep1 19.6μL 1999.2μLTaqPolymerase 0.4μL 40.8μLTotal 20μL 2040μL
TaqPolymerase-LoadedMasterMix:HLA-DQB1Set3Reagent Volume/sample/locus Volume/96samples/locusMasterMixfromStep1 19.2μL 1958.4μLTaqPolymerase 0.8μL 81.6μLTotal 20μL 2040μL
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2.2 -Briefly vortexand spindownall TaqPolymerase-loadedMasterMixes.Aliquot20μLofeachTaqPolymerase-loadedMasterMixintoseparatewellsof96-wellPCRplates.
Note:Class IandClass IIamplificationhavebeenoptimizedusing twodifferentPCRconditions,soClassIandClassIIMasterMixesshouldnotbeinthesameplate.
2.3–Add5μLof eachdilutedgDNA into theappropriatewell of theplatesprepared in thepreviousstep.Mixbypipetting.Seal themwitha thermalsealandvisually inspecteachwell.Spin-downallAmplificationPlatesinacentrifuge.2.4 -Place theAmplificationPlates into thermalcyclersandrun theprograms forClass IandClassIIamplificationaccordingtothetablesbelow:
ClassIAmplification(HLA-A,BandC)NumberofCycles Temperature Time
1 95°C 3minutes 95°C 15seconds
35 65°C 30seconds 68°C 5minutes1 68°C 10minutes1 4°C ∞
ClassIIAmplification(HLA-DRB1andDQB1)NumberofCycles Temperature Time
1 95°C 3minutes 93°C 15seconds
35 60°C 30seconds 68°C 9minutes1 68°C 10minutes1 4°C ∞
Note: Amplification success canbe verified by running 2 μL from each amplicon in astandard2%agarosegelat250Vfor30minutes.(Optional)
ExpectedAmpliconSizes
HLAlocus Expectedampliconsize(kb)HLA-A,BandC ~3HLA-DRB1 ~4.3
HLA-DQB(Set3) ~6.6Safestoppingpoint.Ampliconscanbestoredat4°Covernightorat-20°Cforlonger.
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Step 3 – Amplicon Quantitation and Normalization(usingaPlateFluorometer)Duration:~1hourAmplicon Quantitation and Normalization is recommended to ensure precise input into thelibrarypreparationstep(Optional).AmpliconconcentrationismeasuredusingtheQuantiFluordsDNA System that contains a fluorescent DNA-binding dye and DNA standard for sensitivequantitation of small amounts of double-stranded DNA (dsDNA). Refer to Appendix 2 forInstructionsonhowtodotheAmpliconQuantitationusingaqPCRmachine.
Quick tip – The amplicon quantitation, while recommended, is not required tosuccessfullycompletetheHolotypeHLAprotocol.Ampliconnormalizationdoesnotrequireprecisemeasurementofampliconconcentration.Anestimateofampliconconcentrations based on experience or agarose gel electrophoresis can be usedinstead. Amplicon quantitation should not be skipped without consistentexperiencewiththecompleteHolotypeHLAprotocol.
ReagentlistItem Storage SuppliedbyClassIAmplificationPlate(s) 4°C Step2ClassIIAmplificationPlate(s) 4°C Step2LambdaDNAStandard(100ng/μL) 4°C PromegaQuantiFluordsDNADye(200×) 4°C Promega20×TEBuffer(pH7.5) 4°C PromegaMoleculargradeH2O 20°Cto25°C UserExoSAP-iTExpress -20°C Affymetrix
Protocol3.1 – Prepare DNA standards by serial dilution of the Lambda DNA standard (100 ng/μL)
providedintheQuantiFluorkitaccordingtothedilutiontablebelow:
Labelontube InputDNA VolumeDNA(μL)
Volume1xTE(μL)
FinalConc.(ng/μL)
Standard1 LambdaDNA 7.5μL 492.5μL 1.5ng/μLStandard2 Standard1 250μL 250μL 0.75ng/μLStandard3 Standard2 250μL 250μL 0.38ng/μLStandard4 Standard3 250μL 250μL 0.19ng/μLStandard5 Standard4 250μL 250μL 0.09ng/μLStandard6 Standard5 250μL 250μL 0.05ng/μLBlank Blank 0μL 250μL 0 ng/μL
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3.2 -PreparetheAmpliconQuantitationplates(seesupplementalfigures).Aliquot99μL1xTE
buffer to the wells of a 96-well optical plate for the total number of amplicons to bequantitated.
3.3 -Add1μLofampliconsfromcorrespondingwellsintheAmpliconPlatestoindividualwellsintheAmpliconQuantitationPlates.Mixbypipetting
3.4 - Prepare 1× QuantiFluor Dye working solution using the following formula: 0.5 μLQuantiFluor Dye (200X) + 99.5 μL 1× TE buffer. Prepare sufficient 1× QuantiFluor Dyeworkingsolutionsothateachsample(totalsamplesinAmpliconPlates)andstandard(14total)willreceivea100μLaliquot.
3.5 -PrepareaStandardsQuantitationPlateandAmpliconQuantitationplates.Aliquot100μLof1×QuantiFluorDyeworkingsolutiontowellsofthe96-wellopticalplatethatwillbetheStandardsQuantitationPlateandtotheAmpliconQuantitationPlatesfromStep3.2.
3.6 - Using the standards prepared above, add 100 μL of each standard, in duplicate, to
individualwellsintheStandardsQuantitationPlate(14wellstotal).Mixbypipetting.
3.7 -Vortexwelltomixandspindown.3.8 -RuntheStandardsQuantitationPlateontheplatefluorometerfollowedbytheAmplicon
QuantitationPlates.3.9 -Calculate theconcentrationofDNA in theAmpliconQuantitationPlatesusingRFUdata
generatedbytheplatefluorometer.RefertotheDilutionTabintheprovidedworkbookforassistancewithcalculations.
3.10 - Dilute DNA in the Amplicon Plates with molecular grade H2O so that the final
concentrationofDNAisapproximately67ng/μL.§ IfDNAconcentrationis150ng/μLorgreater:add25μLofH2O§ IfDNAconcentrationis100-150ng/μL:add10μLofH2O§ IfDNAconcentrationislessthan100ng/μL:donotaddanyH2O
Ampliconpooling3.11 - Pool all loci for each sample into a single Pooled Amplicons Plate. Combine thevolumesindicatedforeachlocusasinthefollowingtabletoobtainafinalvolumeof25μL.
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HLAlocus Pooledvolume
A 5μLB 5μLC 5μL
DRB1 5μLDQB1set3 5μL
3.12 – Add 4 μL of ExoSAP-iT Express into each pooled amplicon. Rinse the pipette tips bypipetting.Sealtheplatewithathermalsealandspindown.3.13-PlacethePooledAmpliconsPlateintoathermalcyclerandrunthefollowingprogram:
ExoSAP-ITExpressPCRPurification
NumberofCycles Temperature Time1 37°C 4minutes1 80°C 1minutes1 4°C ∞
Safestoppingpoint.Ampliconscanbestoredat4°Covernightorat-20°Cforlonger.
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Step4–LibraryPreparationDuration:~3hoursDuringthisstep,thepooledampliconsarepreparedforsequencingontheIlluminaMiSeq.Theampliconsareenzymatically fragmented, theendsare repairedandadenylated, and indexedadaptorsareligatedtotheends.ThelibrariesarethenpooledfollowedbyasinglecleanupandconcentrationstepperformedusingAMPureXPbeads.
Note:Omixonrecommendsvolumesgreaterthanisnecessaryfor96samplesbecausemanyoftheenzymesandbuffersareviscous,resultinginexcesspipettingloss.
ReagentlistItem Storage SuppliedbyPooledAmpliconsPlate 4°C Step3FragmentationEnzyme(A) -20°C OmixonFragmentationBuffer(B) -20°C OmixonEndRepairEnzyme(C) -20°C OmixonEndRepairBuffer(D) -20°C OmixonLigationEnzyme(E) -20°C OmixonLigationBuffer(F) -20°C OmixonAdaptorPlate -20°C OmixonAMPureXPbeads 4°C BeckmanCoulter80%Ethanol(freshlyprepared) 20°Cto25°C UserMoleculargradeH2O 20°Cto25°C User
Protocol4.1-Turnonthethermalcycler.Verifythattheheatedlidiswarmingup.
Note:BesuretovortextheFragmentationEnzyme(A)thoroughlybeforeuse.4.2-PrepareFragmentationMasterMixaccordingtothetablebelow:
FragmentationMasterMix
Reagent Volumeperlibrary(μL)
Recommendedvolumesfor96libraries(μL)
Colorcode
FragmentationEnzyme(A) 2μL 220.8μL YellowFragmentationBuffer(B) 2μL 220.8μL RedTotalVolume 4μL 441.6μL
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4.3-PrepareaReagentPlate:placeanew96-wellPCRplateonaPCRcoolerrackandaliquotandequalamountoftheFragmentationMasterMixintoeachwellofasinglecolumn.
Note:Thefragmentationreactionhasbeendesignedtoprovide ideallysizedDNAforsequencingonthe IlluminaMiSeq. It is important tokeepthereagentscolduntil thereaction is started in the thermal cycler to prevent excessive fragmentation. Use ofmulti-channel pipettes is recommended to minimize opportunities for excessivefragmentation.
4.4-CentrifugethePooledAmpliconsPlatefor10seconds,andplaceitoniceoracoldblock.4.5-PrepareaReactionPlate:placeafresh96-wellPCRplateonaPCRcoldblock.4.6-Add4μLofFragmentationMasterMixfromtheReagentPlateintowellsoftheReactionPlate, correspondingwith samples in thePooledAmpliconsPlate.Theuseofamulti-channelpipetteisrecommended.4.7 -Transfer16μLofeachamplicon fromthePooledAmpliconsPlate to thecorrespondingwellontheReactionPlateusingamulti-channelpipette.Mixbypipetting.4.8-CovertheReactionPlatewithathermalsealandcentrifugefor10seconds.4.9-IncubatetheReactionPlateinathermalcyclerwiththefollowingprogram:
FragmentationProgram
NumberofCycles Temperature Time1 37°C 10minutes1 70°C 15minutes1 4°C ∞
Safestoppingpoint.Librariescanbestoredat4°Covernightorat-20°Cforlonger.
4.10-PreparetheEndRepairMasterMixaccordingtothetablebelow:
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EndRepairMasterMix
Reagent Volumeperlibrary(μL)
Recommendedvolumesfor96libraries(μL)
Colorcode
MoleculargradeH2O 1.25μL 139.2μL EndRepairEnzyme(C) 1.25μL 139.2μL GreenEndRepairBuffer(D) 2.5μL 278.4μL OrangeTotalVolume 5μL 556.8 μL 4.11-AliquotanequalamountofEndRepairMasterMix intoasingleunusedcolumnoftheReagentPlate.4.12-CentrifugetheReactionPlate(containingthefragmentedSamples)for10seconds.Add5μLofEndRepairMasterMixfromtheReagentPlateintoeachwelloftheReactionPlate.Theuseofamulti-channelpipetteisrecommended.Mixbypipetting.4.13-CovertheReactionPlatewithathermalsealandcentrifugefor10seconds.4.14-IncubatetheReactionPlateinathermalcyclerwiththefollowingprogram:
EndRepairProgram
NumberofCycles Temperature Time1 20°C 30minutes1 70°C 5minutes1 4°C ∞
Safestoppingpoint.Librariescanbestoredat4°Covernightorat-20°Cforlonger.
4.15-Removethe IndexedAdaptorsPlatefromstorageandthawatroomtemperatureafterthe End Repair Program starts in the thermal cycler. When the Adaptor Plate is at roomtemperature,centrifugeitfor3minutesat3000rpm.4.16-CarefullypullthesealoffoftheAdaptorPlate.DonotshaketheAdaptorPlateoncethesealisremovedtopreventcrosscontamination.4.17 – Transfer the entire volume of each well from the Reaction Plate (25 μL) to thecorrespondingwellintheAdaptorPlate.
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Note: IftheentireAdaptorPlateisNOTgoingtobeused, it ispossibletouseonlythenecessarynumberofadaptors.Cuttheplatesealbetweenthewellstobeusedand thewells tobekept.Carefullypull the sealoff theAdaptorPlate, leaving thesealinplaceoverthewellstobekept.a. Transfer25μLfromeachend-repairedsampleoftheReactionPlatetoawellin
theAdaptorPlate,mixingwellwithapipette.
b. TransfertheentiretyofeachsamplefromtheAdaptorPlateintotheoriginalwelloftheReactionPlate.
c. ResealtheAdaptorPlateandreturnitto-20°C.UsetheReactionPlateinsteadoftheAdaptorPlatefortheremainingstepsinthemanual.
4.18-PreparetheLigationMasterMix.PrepareenoughLigationMasterMixforeachsample.
LigationMasterMix
Reagent Volume(μL) Recommendedvolumesfor96libraries(μL)
Colorcode
LigationEnzyme(E) 2.5μL 252.5μL BlueLigationBuffer(F) 30μL 3030μL BlackTotalVolume 32.5 3282.5μL
4.19-AliquottheLigationMasterMixinto3unusedcolumnsoftheReagentPlate.Theuseofamulti-channelpipetteisrecommended.4.20 -Add32.5μLof LigationMasterMix intoeachwell of theReactionPlate. Theuseof amulti-channelpipetteisrecommended.Mixbypipetting.4.21-CovertheReactionPlatewithathermalsealandcentrifugefor10seconds.4.22-IncubatetheReactionPlateinthethermalcyclerwiththefollowingprogram:
LigationProgramNumberofCycles Temperature Time
1 25°C 10minutes1 70°C 10minutes1 4°C ∞
Safestoppingpoint.Librariescanbestoredat4°Covernightorat-20°Cforlonger.
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Poolingandlibrarypurification4.23-AllowAMPureXPbeadstocometoroomtemperature.Ensuretheyarehomogeneous(noclumpsorpellets).Preparefreshlymade5mLof80%ethanol(4mLEtOH+1mLH2O).4.24-CreatetheLibrarybycombininganaliquotfromeachpooledamplicon,nowasample-specificlibrary,intoasingle2.0mLlowbindmicrocentrifugetube.
I. For 16 ormore samples - Calculate the amount of each sample library to pooltogetherasasingleLibraryof900μLtotalvolume.Divide900μLbythenumberofsamplelibraries.ThisisthevolumeofaliquottobetakenfromeachsamplelibraryandpipettedintotheLibrary.
II. Forfewerthan16samples–Transfer60μLofeachsamplelibraryintoaLibrary.4.25 -Add900μLofAMPureXPbeads to theLibrary tube.Mix thoroughlybyvortexingandcentrifugebriefly.Donotallowthebeadstoseparate. IncubatetheLibrary for10minutesatroomtemperature.
Note: If there is less than 900 μL of library in the Final Pool, add an equivalentamountofAMPureXPbeads.Thereshouldbea1:1ratioofFinalPoolandAMPureXPbeads.
4.26-PlacetheLibrarytubeontoamagneticstandandincubatefor10minutes.4.27–Keepingthetubeonthemagneticstand,carefullyremoveanddiscardthesupernatantfromtheLibrarytube,withouttouchingthebeads.4.28-Keepingthetubeonthemagneticstand,add~1.5–2mLoffreshlyprepared80%ethanoltotheLibrarytube.Thevolumeofethanoladdedshouldbesufficienttocoverthebeads.
Note:Applytheethanoltothesideofthetubewithoutbeads.4.29 - Incubate the Library tube at room temperature for 30 seconds; afterwards, carefullyremoveanddiscardthesupernatant.4.30-Repeatsteps4.28and4.29.4.31-QuicklyspindowntheLibrarytubeandplaceitbackonthemagneticstandwiththelidopen.Removeresidualethanolwithapipette.Donottouchthebeads.
Note: Ensure the bead pellet does not contain residual ethanol. This may requirerotating the tubeon themagnetic stand to removeethanolwithoutdisturbing thebeadpellet.
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4.32-Allowthebeadstoairdryfor5-8minutesonthemagneticstanduntilthebeadpelletisdry.4.33 - Remove the Library tube from the magnetic stand and elute the Library with 31 μLmoleculargradewater.Donotletthepipettetiptouchthebeads,astheywillsticktoit.4.34 - Vortex the Library to fully resuspend the beads. Centrifuge briefly if some dropletsremainonthesidewalls.Ensurethebeadsremaininsuspension.4.35-IncubatetheLibraryatroomtemperaturefor2minutes.4.36-PlacetheLibrarytubeonthemagneticstandfor2minutes.4.37-CollecttheLibrary:keepingtheFinalLibrarytubeinthemagneticstand,collect31μLofthesupernatantintoanew1.5mllowbindmicrocentrifugetube.
Safestoppingpoint.Librariescanbestoredat-20°Cforextendedperiodsoftime.
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Step5–LibrarySizeSelectionDuration:~1hourStep 5 takes the Library from Step 4 and performs size selection using the Pippin Prep. ThePippin Prep can automatically select a range of DNA fragment sizes and elute them into acollection chamber. Note: Blue Pippin may be used instead of the Pippin Prep. Refer toAppendix1forPippinPrepInstructionsforUse.
ReagentlistItem Storage Suppliedby1.5%AgaroseGelCassette,DyeFree 20°Cto25°C SageSciencePippinloadingsolution/markermix(labeledK)
4°C SageScience
PooledLibrary 4°C Step4Note:MarkerKisusedwiththePippinPrep.TheBluePippinusesMarkerR2.
Protocol5.1-BringtheMarkerKloadingsolutiontoroomtemperature.5.2-Combine31μLofthePoolwith10μLofMarkerKloadingsolution.5.3-Mixbyvortexingandspindown.5.4-ConfigurethePippinPreptocollectDNAfragmentsbetween650and1300bps.Loadthe40μLsampleintothesampleportandrun.Runtimeis45-50minutes.5.5-Collectthewholecontent(approximately40μL)fromtheelutionportofthePippinPrepandtransferittoanew1.5mllowbindmicrocentrifugetube.Thisisthesize-selectedlibrary.
Safestoppingpoint.Librariescanbestoredat-20°Cforextendedperiodsoftime.
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Step 6 – Library Quantification using an intercalatingdsDNAfluorescentdyeDuration:~15minutesIt isnecessarytoquantifythesize-selectedlibrary inordertooptimallyusetheoutputoftheIllumina MiSeq sequencer. The concentration of the size-selected library can be accuratelymeasured by an intercalating dsDNA fluorescent dye, such as SYBR green or equivalent.Commerciallyavailablekitsandinstrumentsforthispurposeinclude,butarenotlimitedto,theQubit reader by Thermo Fisher (uses the Qubit Broad-Range dsDNA assay kit), the QuantusreaderbyPromega(usestheQuantifluordsDNAfluorescentdye)andothers.Here,theQubitmethod isdescribedas it isthemostcommonlyused instrument. Incaseanother instrumentandkitisused,followthemanufacturer’sstandardinstructions.
Note: This dsDNA fluorometric method is a quick but accurate enough way todeterminetheconcentrationof thefinalsize-selected library. Itmeasuresallof thedsDNA that is present in the library.Optionally youmay use the KAPA BiosystemsLibraryQuantitationkitandqPCRmachine foramorespecificmeasurementof thelibraryconcentration.ForthisprotocolSeeAppendix3.
ReagentlistItem Storage SuppliedbyQubitdsDNABRAssayKit roomtemperature ThermoFisherQubitdsDNABRStandards 4°C ThermoFisherSizeSelectedLibrary 4°C Step5
Protocol6.1–BringtheQubitStandardstoroomtemperature.PrepareQubitassaytubes(500µL,thin-
walled) for your library in duplicate and the two standards. Vortex and centrifuge thestandardsandthelibrary.
6.2–Add995µL fromBufferand5µL fromdyetoa1.5mlcentrifugetube.Vortexandspin
down.
6.3–Transfer190µL fromthereagentmixtotheQubittubesforthetwostandards.Transfer198µL fromthereagentmixtothetwoQubittubesfortheduplicatesofthelibrary.
6.4–Add10µLfromstandard1tothecorrespondingQubittubeandvortexitfor2seconds.Repeatwithstandard2.
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6.5–Add2µL fromthelibrarytothecorrespondingQubittubesandvortexfor2seconds.
6.6–IncubatetheQubittubesatroomtemperaturefor2minutes.
6.7–SwitchonQubitmachineandchooseBRprotocol.6.8–Putstandard1QubittubeinandpushGO.Repeatwithstandard2.6.9–PutthelibrarytubeinQubitandpushGO.Repeatforthereplicate.6.10 – To convert the Qubit result from ng/μL to nM concentration, enter the meanconcentration of the two library replicates in the Omixon Workbook tab called “LibraryQuantitation”.6.11–UsingtheresultsfromtheQubitmeasurement,dilute10μLoftheSizeSelectedLibrarytoaconcentrationof2nMwithsterileH2O ina fresh1.5-mL lowbindmicrocentrifuge tube.StoretheremainingSizeSelectedLibraryat-20°C.
Safestoppingpoint.Librariescanbestoredat-20°Cforextendedperiodsoftime.Incase of long-term storage, re-quantification of the library is highly recommendedbeforerunningitontheMiSeq.
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Step7–SequencingonIlluminaMiSeqDuration:~24-40hoursThe Illumina MiSeq is an automated NGS instrument that can sequence the Size-selectedLibrary prepared in the previous steps. De-multiplexing of the indexed samples is doneautomaticallyfollowingcompletionofthesequencingrun.
Quicktip–Youcanusea1%PhiXspike-inasanadditionalcontrol tomonitor thesequencing reaction. Refer to Illumina documentation on the PhiX control foradditionalinformation.
ReagentlistItem Storage SuppliedbyReagentCartridge -20°C IlluminaHT1 -20°C IlluminaPR2 4°C IlluminaMiSeqFlowCell 4°C IlluminaLibraryat2nM 4°C Step6NaOH1Nor2N 20°Cto25°C UserMoleculargradeH2O 20°Cto25°C User
MiSeqReagentKitcapacityIlluminaMiSeqReagentKit
TimeHours
24/7Samples
24/11Samples
96/5Samples
96/7Samples
96/11Samples
Std300Cycle(MS-102-2002)
~24 24 24 96 96 72
Micro300Cycle(MS-103-1002)
~19 24 20 40 28 20
Nano300Cycle(MS-103-1001)
~17 6 4 8 6 4
Std500Cycle(MS-102-2003)
~39 24 24 96 96 96
Nano500Cycle(MS-103-1003)
~28 12 8 16 12 8
Protocol7.1-PreparetheMiSeqaccordingtostandardIlluminaprotocols.7.2-Preparea1nMDenaturedLibrary:Combine10μLoffreshlyprepared0.2NNaOHand10μLof the2nMDilutedSizeSelectedLibrary inanew1.5mL lowbindmicrocentrifuge tube.
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Vortex and spin down. Incubate this 1 nM Denatured Library at room temperature for 5minutes.7.3-Preparea20pMDenaturedLibrary:Add980μLofchilledHT1tothe20μLofthe1nMDenaturedLibrary.Vortexandspindown.7.4 -Preparea9pMDenaturedLibrary:Add550μLofchilledHT1and450μLof the20pMDenaturedLibrarytoafresh1.5mLlowbindmicrocentrifugetube.Vortexandspindown.7.5 – Transfer 600μLof the9pMDenatured Library into the Load Samples reservoir of theMiSeqreagentcartridge.
Quicktip–ItisadvisabletousetheprovidedworkbooktocreatetheSampleSheetthatisrequiredbytheMiseq.EnsurethatthecorrectAdaptorPlateconfiguration(Aor B) is selected on the Omixon Workbook Sequencing tab that contains theappropriateindexedadaptorsequences.
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Step8–AnalysisofHLASequencingDataTheIlluminaMiSeqwillprocessthe9pMPooledLibraryandgeneratesequencingdataasfastqfiles. Please refer to theHLATwinmanual for assistancewith the correct installationofHLATwinandforinformationoninterpretingthegenotypinganalysisofyoursequencingdata.Forimplementing the Automated Protocol and issues relating to installation or analyzing data,[email protected].
AutomatedProtocol
ITSetupandConfiguration1. InstallHLATwinServerontheServer2. InstallHLATwinClientonaclientcomputer–multipleHLATwinClientsmayconnectto
theserver3. ContactOmixonSupport([email protected])forcustominstallationinstructionsfor
Automation
ProtocolperAnalysis1. LaunchHLATwinClientandlogin2. Data is already processed or is being processed. Review the results using the Traffic
LightSysteminHLATwin3. Exportthegenotypingresultsand/orconsensussequencesasrequired
ManualServerProtocol
ITSetupandConfiguration1. InstallHLATwinServerontheServer2. InstallHLATwinClientonaclientcomputer
ProtocolperAnalysis1. LaunchHLATwinClientandlogin2. SelecttheMiSeqdatainfastqorfastq.gzformatandstarttheHolotypeHLAtypingrun3. After the Holotype HLA typing has finished, review the results using the Traffic Light
SysteminHLATwin4. Exportthegenotypingresultsand/orconsensussequencesasrequired
ManualDesktopProtocol
ITSetupandConfiguration1. InstallHLATwinDesktop.
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ProtocolperAnalysis1. LaunchHLATwinandlogin2. SelecttheMiSeqdatainfastqorfastq.gzformatandstarttheHolotypeHLAtypingrun3. After the Holotype HLA typing has finished, review the results using the Traffic Light
SysteminHLATwin4. Exportthegenotypingresultsand/orconsensussequencesasrequired
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TechnicalAssistanceForgeneralassistancewiththisprotocolcontactsupport@omixon.comSafetyDataSheetsareavailableatwww.omixon.com/holotype-hla-documentation/msds
PhoneSupport:UnitedStates|+1(617)500-0790Europe|+36705748001RestofWorld|+1(617)500-0790
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SupplementalFigures
PlateexampleforAmpliconPlate,AmplificationPlate,DilutionPlate,AmpliconQuantitationPlate(foranindividuallocus)&ReactionPlate
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StandardsQuantitationPlateExample
KAPALibraryQuantitationqPCRPlateExample
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Appendix1:PippinPrep
ProgrammingthePippinPrep1. ClicktheProtocolEditorTabandclickthe“New”button.
2. ClickthefoldericonnexttotheCassettefieldandselect“1.5%DFMarkerK”forthePippinPrepor“1.5%DFMarkerR2”fortheBluePippin.
3. Inthelanethatyouareprogramming:
a. Highlightthe“Range”field.b. Setthe“RefLane”tomatchthelanenumberyouareworkingin.c. Setthe“Start*”fieldto650.d. Setthe“End*”fieldto1300.
4. IntheReferenceLanefield,selectthelanethatyouareworkingin.
5. Clickthe“SaveAs”buttonandnameyourprogram.
RunningthePippinPrep1. TurnonthePippinPrepbypushingthepowerbuttoninthebackofthedevice.
2. Visually inspect thePippinPrep.Make sure the5 LEDsareonand that the insideof thedeviceiscleananddry.
3. Click on the Sage Science logo on the bottom right of the screen. Thiswill allow you toenterapassword.Thefactorydefaultpasswordis“pips”.
4. ClicktheFactorySetupTabandmakesuretheBase-to-Thresholdvalueissetto0.02.
5. PlacethecalibrationfixtureinsidethePippinPrep,makingsurethedarkstripisfacedownandovertheLEDlights.
6. IntheMaintab,clickthe“Calibration”button.
7. IntheCalibrationwindow,makesurethe“TargetIpHmA”fieldissetto0.80(0.60forBluePippin)andthenhitthe“Calibrate”button.
8. GototheProtocolsTab.Clickthe“Load”buttonandselecttheprogramforHolotypeHLAandthespecificlaneyouwillbeusing.Makesurethat:
a. Thecorrectlaneisturnedon
b. Broadspectrumselectionindicatorison
c. Thereferencelaneisthesamelanethatwillberunning.
9. GototheMainTab.Makesurethat:
a. Theprogramyouloadedistheonethatisselected.
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b. Theappropriatereferencelaneisselectedandthatitisalsothelanethesamplewillberunin.
10. Inspect thecassette.Beforetakingoff thetapesealing thewells, looktosee if thereareany bubbles behind the elution port. If there are any bubbles behind the elution port,gentlytapandrollthecassetteinyourhandtoworkthebubblesout.
11. Placethecassette,withthetapestilloverthewells,insideofthePippinPrep.
12. Carefully peel off the tape,making sure to remove the tape from the clean side of thecassette (lane5) to theused sideof the cassette (lane1). Take carenot to splash liquidwhenthetapeisremovedtopreventcontamination.
13. Removetheentirevolumeofbufferfromtheelutionportofthelaneyouwillbeusingandadd40μLoffreshelectrophoresisbufferinthatelutionport.
14. Addathinstripoftapeovertheelutionports.
15. Any reservoirs that are less than 3/4ths full should be topped off with electrophoresisbuffer.Donotoverfillthewells!Theedgeofthebuffershould‘just’reachtheplasticnothighertopreventdraggingwhenthelidslides.Applybufferfromthecleanwells(Lane5)totheusedwells(Lane1).
16. Make sure each of the loadingwells (wells with agarose) are filledwith electrophoresisbuffer.Thebuffershouldbe‘just’overtheagarose,appearingcompletelyflat.
17. ClosethePippinPrepslowly,watchingtomakesurenobufferistouchingthelidasyouareclosingthedevice.
18. Perform the continuity test. When the sensors dry out slightly, it is common for thecontinuitytesttofailonce.Ifthecontinuitytestfails,runthetestonemoretime.Oncethecontinuity test completes, open the Pippin slowly. Make sure no fluid is getting pulledacrossthecassettebythelidofthePippinPrep.
19. Briefly vortex the Marker K loading solution and spin it down. Add 10 μL of Marker Kloadingsolutiontoyour~30μLoflibrary.
20. Brieflyvortexyourlibraryandspinitdown.
21. Remove40μLofbufferfromthesamplewellthatyouwillbeusing.
22. Add~40μLofyourlibraryloadedwithMarkerKtothesamplewellthatyouwillbeusing.
23. Markthelanethatyouareusingwiththetechnician’sinitialsandthedate.
24. Close the Pippin Prep and click the “Start” button.Make sure the appropriate lane hasbeenturnedon.Thesampleshouldrunforabout45minutes.
25. Aftertherunhascompleted,carefullyopenthePippinPrep.Watchtoseeiftheliddragsanyliquidacrossthecassette.
26. Removethetapeovertheelutionports,beingcarefulnottoflickanyliquid.
27. Transferallthevolumefromtheelutionportintoanew1.5mllowbindtube.
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28. Coveralloftheopenwellswithtwopiecesofplatesealingtape.Remembertoleaveatabonthecleanside.Thiswillmakeitsimpletoremovethetapefromcleantoused.
29. Placethesealedcassetteintoitsbagandsetitaside.
30. TakethewashcassetteandfillitwithMiliQwater.GentlyclosethelidofthePippinPrep,watchingtoseeifyoupullanyliquidacrossthewashcassette.
32. LeavethePippinPrepclosedforseveralseconds.
33. OpenthePippinPrep,watchingtoseeifyoupullanyliquidacrossthewashcassette.
34. Removethewashcassette,emptyitofwater,andletitdry.
35. CleananywateroffofthePippinPrepandcloseitgently.
36. Selectthe“ShutDown”buttoninthePippinPrepmenu.
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Appendix 2: Amplicon Quantitation using a qPCRinstrumentDuration:~1hours
ReagentlistItem Storage Suppliedby20×TEBuffer(pH7.5) 4°C PromegaLambdaDNAStandard(100ng/μL) 4°C Promega200×QuantiFluordsDNADye 4°C PromegaSterileH2O 20°Cto25°C UserClassIAmplificationPlate(s) 4°C Step2ClassIIAmplificationPlate(s) 4°C Step2
Protocol1. Createaserialdilutionusing1.5mLmicrocentrifugetubesandtheQuantiFluorLambda
DNAstandard(100ng/μL).Followthedilutiontablebelow:
Labelontube InputDNA VolumeDNA(μL)
Volume1xTE(μL)
FinalConc.(ng/μL)
Standard1 LambdaDNA 7.5μL 492.5μL 1.5ng/μLStandard2 Standard1 250μL 250μL 0.75ng/μLStandard3 Standard2 250μL 250μL 0.38ng/μLStandard4 Standard3 250μL 250μL 0.19ng/μLStandard5 Standard4 250μL 250μL 0.09ng/μLStandard6 Standard5 250μL 250μL 0.05ng/μLStandard7,Blank
Blank 0μL 250μL 0ng/μL
2. PreparetheAmpliconQuantitationplates(seesupplementalfigures).Aliquot49.5μL1x
TEbuffertothewellsofaclean96-wellplateforthetotalnumberofampliconstobequantitated.
3. Add0.5μLofampliconsfromcorrespondingwells intheAmpliconPlatesto individualwellsintheAmpliconQuantitationPlates.Mixbypipetting.
4. Prepare 1× QuantiFluor Dye working solution using the following formula: 0.25 μLQuantiFluorDye(200X)+49.75μL1×TEbuffer.Preparesufficient1×QuantiFluorDyeworkingsolutionso thateachsample (total samples inAmpliconPlates)andstandard(14total)willreceivea50μLaliquot.
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5. PrepareaStandardsQuantitationPlateandAmpliconQuantitationplates.Aliquot50μLof1×QuantiFluorDyeworkingsolutiontowellsofthe96-wellopticalplatesusingtheformatof theStandardsQuantitationPlateandtheAmpliconQuantitationPlates (seesupplementalfigures).
6. Using the standards prepared above, add 50 μL of each standard, in duplicate, toindividualwellsintheStandardsQuantitationPlate(14wellstotal).
7. Vortextomixthoroughlyandspindown.
8. PuteachQuantitationPlate in theqPCRmachineoneata timeandrun the followingprogram:NumberofCycles Temperature Time
1 25°C 10seconds 25°C 15seconds2 25°C 30seconds(dataacquisition)
9. CalculatetheconcentrationofDNA in theAmpliconQuantitationPlatesusingtherawRFUdatageneratedbytheqPCRinstrument.
10. DiluteDNA in the Amplicon Plateswith sterile H2O so that the final concentration ofDNAisapproximately67ng/μL.
§ IfDNAconcentrationis150ng/μLorgreater:add25μLofH2O
§ IfDNAconcentrationis100-150ng/μL:add10μLofH2O
§ IfDNAconcentrationislessthan100ng/μL:add0μLofH2O
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Appendix 3: Library Quantitation using a qPCRinstrumentDuration:~1hourItisnecessarytoquantifytheSize-selectedLibraryinordertooptimallyusetheoutputoftheIllumina MiSeq sequencer. The concentration of the Size-selected Library can be accuratelymeasuredbyqPCR.
ReagentlistItem Storage Suppliedby10×IlluminaPrimerPremix -20°C KAPABiosystems2×KAPASYBRFASTqPCRMasterMix -20°C KAPABiosystemsStd1(20.00pM) -20°C KAPABiosystemsStd2(2.00pM) -20°C KAPABiosystemsStd3(0.20pM) -20°C KAPABiosystemsStd4(0.02pM) -20°C KAPABiosystemsIlluminaDNAStandards -20°C KAPABiosystemsMoleculargradeH2O User1×TEBuffer(pH8.0) UserSizeSelectedLibrary 4°C Step5
Protocol1-PreparetheqPCRPrimerMixusingthe10×IlluminaPrimerPremixandthe2×KAPASYBRFASTqPCRMasterMix:
Note:TheKAPASYBRFASTqPCRkitreagents(qPCRMasterMix,PrimerPremixandROXsolutions)arecombinedduringthefirstuseofthekit.Thiscombinedsolutionisstableforatleast30freeze/thawcycles.FollowKAPAdocumentationtodetermineifROXisrecommendedforyourqPCRinstrument.
qPCRPrimerMix
Reagent Volume(mL)10×IlluminaPrimerPremix 1mL2×KAPASYBRFASTqPCRMasterMix 5mLTotalVolume 6mL2–PreparetheqPCRMasterMix.
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qPCRMasterMix
Reagent Volume(μL)qPCRPrimerMix 228μLMoleculargradeH2O 76μLTotalVolume 304μL3-PrepareaserialdilutionoftheSizeSelectedLibrary.
a. Preparea1:1000dilutionbyadding1μLofSizeSelectedLibrary to999μLof1×TEbuffer(pH8.0),thoroughlyrinsingthepipettetip.Vortexandspindown.
b. Prepare a 1:2000 dilution by adding 100 μL of the 1:1000 dilution to 100 μL 1× TEbuffer(pH8.0).Vortexandspindown.
4-PrepareaqPCRQuantitationPlateinafreshPCRplatecompatiblewithyourqPCRsystem.5-Aliquot16μLoftheqPCRMasterMixintriplicateforstandards1-4,the1:1000dilutionand
the1:2000dilution(seesupplementalfigures).6 - Aliquot 4 μL of standards 1-4, the 1:1000 dilution and the 1:2000 dilution into the
correspondingwells.7-SealtheqPCRQuantitationPlateandcentrifugeitfor10seconds.
Note: Avoid creating bubbles in the qPCRQuantitation Platewells. Centrifuge asneededtoeliminatebubbles.
8 -Setthe1:1000and1:2000triplicatesastargetedsamples,anddefinethestandards(points:4, starting concentration: 20pM, dilution: 1:10). Run the following program on the qPCRmachineinordertodeterminetheDNAconcentrationoftheSizeSelectedLibrary:
NumberofCycles Temperature Time1 95°C 5minutes25
(nomeltcurve)95°C 30seconds60°C 90seconds(dataacquisition)
9 – To convert the qPCR result from pM to nM concentration, enter the “Quantity mean”resultsofthetwolibraryreplicatesintheOmixonWorkbooktabcalled“LibraryQuantitation”.
10 -Using thevolumes fromtheworkbook,dilute10μLof theSizeSelectedLibrary toaconcentrationof2nMwithsterileH2Oinafresh1.5-mLlowbindmicrocentrifugetube.StoretheremainingSizeSelectedLibraryat-20°C.
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Safestoppingpoint.Librariescanbestoredat-20°Cforextendedperiodsoftime.Incase of long-term storage, re-quantification of the library is highly recommendedbeforerunningitontheMiSeq.