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REGULAR ARTICLE Severe platelet dysfunction in NHL patients receiving ibrutinib is absent in patients receiving acalabrutinib AlexanderP.Bye,1AmandaJ.Unsworth,1MichaelJ.Desborough,2,3CatherineA.T.Hildyard,4NiamhAppleby,4,5DavidBruce,4,5 NelineKriek,1SophieH.Nock,1TanyaSage,1CraigE.Hughes,1,*andJonathanM.Gibbins1,* 1InstituteforCardiovascularandMetabolicResearch,UniversityofReading,Reading,UnitedKingdom;2OxfordHaemophiliaandThrombosisCentre,OxfordBiomedical ResearchCentre,ChurchillHospital,Oxford,UnitedKingdom;3NuffieldDivisionofClinicalLaboratorySciences,UniversityofOxford,Oxford,UnitedKingdom;4Departmentof Haematology,ChurchillHospital,OxfordUniversityHospitalsNationalHealthServicesFoundationTrust,Oxford,UnitedKingdom;and5DepartmentofOncology,Universityof Oxford,Oxford,UnitedKingdom TheBrutontyrosinekinase(Btk)inhibitoribrutinibinducesplateletdysfunctionandcauses KeyPoints increasedriskofbleeding.Off-targetinhibitionofTecisbelievedtocontributetoplatelet (cid:129)Acalabrutinibpreserves dysfunctionandothersideeffectsofibrutinib.Thesecond-generationBtkinhibitor Srcfamilykinase activ- acalabrutinibwasdevelopedwithimprovedspecificityforBtkoverTec.Weinvestigated ity andavoids dysfunc- plateletfunctioninpatientswithnon-Hodgkinlymphoma(NHL)receivingibrutinibor tional platelet thrombus acalabrutinibbyaggregometryandbymeasuringthrombusformationoncollagenunder formation caused by arterialshear.Bothpatientgroupshadsimilarlydysfunctionalaggregationresponsesto ibrutinib therapy. collagenandcollagen-relatedpeptide,andcomparisonwithmechanisticexperimentsin (cid:129)Platelet thrombus whichplateletsfromhealthydonorsweretreatedwiththeBtkinhibitorssuggestedthatboth formation is enhanced drugsinhibitplateletBtkandTecatphysiologicalconcentrations.Onlyibrutinibcaused by intermediate purity dysfunctionalthrombusformation,whereassizeandmorphologyofthrombifollowing factor VIII. acalabrutinibtreatmentwereofnormalsizeandmorphology.Wefoundthatibrutinibbut notacalabrutinibinhibitedSrcfamilykinases,whichhaveacriticalroleinplateletadhesion tocollagenthatislikelytounderpinunstablethrombusformationobservedinibrutinib patients.Wefoundthatplateletfunctionwasenhancedbyincreasinglevelsofvon Willebrandfactor(VWF)andfactorVIII(FVIII)exvivobyadditionofintermediatepurity FVIII(HaemateP)tobloodfrompatients,resultinginconsistentlylargerthrombi.We concludethatacalabrutinibavoidsmajorplateletdysfunctionassociatedwithibrutinib therapy,andplateletfunctionmaybeenhancedinpatientswithB-cellNHLbyincreasing plasmaVWFandFVIII. Introduction TheBrutontyrosinekinase(Btk)inhibitoribrutinibwasthefirstofanewclassofdrugforthetreatmentof indolentnon-Hodgkinlymphomas(NHLs).1Treatmentwithibrutinibhasproventobeefficaciousbutis associated with side effects, including increased risk of major bleeding.2 Bleeding associated with ibrutinib is potentially explained by off-target inhibition of other kinases in addition to Btk; a study of patientswithX-linkedagammaglobulinemia(XLA),whohaveBtkdeficiency,reportednoincreasedrisk ofbleeding3althoughgeneticdeficiencyofBtkwasfoundtoincreasetimeocclusioninamousemodel ofcarotidarteryinjury.4Furthermore,studiesperformedusinggeneticallymodifiedmicedemonstrated redundancybetweenBtkandTecinplateletsignalingbecauseablationofbothkinaseswasrequiredto Submitted28August2017;accepted7November2017.DOI10.1182/ Thefull-textversionofthisarticlecontainsadatasupplement. bloodadvances.2017011999. ©2017byTheAmericanSocietyofHematology *C.E.H.andJ.M.G.contributedequallytothiswork. 2610 12DECEMBER2017xVOLUME1,NUMBER26 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. Table1.Patientinformation Acalabrutinib100mgBD(n58) Ibrutinib480mgOD(n56) Btkinhibitornaı¨ve(n55) Age,median(range),y 68(53-80) 68(60-77) 78(60-80) Sex,n(%) Female 2(25) 3(50) 3(60) Male 6(75) 3(50) 2(40) Diagnosis,n(%) CLL 7(87.5) 6(100) 5(100) Mantlecelllymphoma 1(12.5) — — Laboratoryparameters Hemoglobin,median(range),g/L 139(113-155) 131(109-147) 140(117-148) Plateletcount,median(range),3109/L 148.5(35-228) 114(58-197) 118(109-274) Clinicaldetails,n(%) Concurrentantiplateletdrugs — — — Concurrentanticoagulants 1(13)* — — Inheritedbleedingdisorders — — — DurationofBtkinhibitor,median(range),mo 21.5(19-32) 19(2-39) — Activebleedingattimeofrecruitment — — — BleedingonBtkinhibitor,n(%)† None 3(38) 5(83) — Grade1 2(25) 1(17) — Grade2 3(38) — — ResponsetoBtkinhibitor,n(%)‡ Completeremission 5(63) 3(50) — Partialremission 3(38) 3(50) — Stableorprogressivedisease — — — BD,twicedaily;OD,oncedaily. *Dabigatran150mgtwicedaily. †CommonTerminologyCriteriaforAdverseEventsgradingscale. ‡InternationalWorkshoponChronicLymphocyticLeukemiacriteriaforchroniclymphocyticleukemia;positronemissiontomographycomputedtomographycriteriaformantlecell lymphoma. renderplateletsfullyinsensitivetocollageninaggregationassays.5 discrepancy between bleeding risk in patients with XLA and The effect of simultaneous genetic ablation of Btk and Tec on patients receiving ibrutinib has not been characterized, but is platelet adhesion under shear has not been explored in vivo or in thoughttorelatetooff-targetinhibitionofTec.8However,ibrutinib vitro.Theoff-targeteffectsofibrutinibonplateletfunctionhaveadded mayalsoinhibit otherimportant plateletkinases such asSFK that complications to its use, such as risks associated with concurrent phosphorylate several signaling molecules in the GPVI signaling treatment with anticoagulant or antiplatelet medication, which is pathway.17BtkandTecarethemselvesdependentonSFK-mediated commonamongpatientswithchroniclymphocyticleukemia(CLL).6 tyrosine phosphorylation to become active.18,19 Inhibition of SFK is Ibrutinib therapy is interrupted before surgery to reduce the risk of known to cause hemostatic dysfunction because the Src inhibitor, bleeding, but prolonged dose interruption or dose reduction may dasatinib,isassociatedwithincreasedbleedingrisk.20-22Comparison reduceefficacyandleadtoaflareinsymptoms.7Acalabrutinibisa ofibrutinibandacalabrutinibtherapythereforerepresentsanimportant second-generationBtk inhibitorand exhibitsgreater selectivity over opportunitytocharacterizetheirrelativeeffectsandunderstandhow kinases that are important for platelet function such as Src family improvedkinasespecificityaffectsplateletdysfunction. kinases(SFKs)and Tec.8 Nomajorbleeding eventswere reported ThrombocytopeniaisfrequentlyassociatedwithCLLandmaybea duringaphase2trialofacalabrutinibfortreatmentofCLL,8butitis contributing factor to bleeding events in combination with drug- notyetcleariftheselectivityofacalabrutinibissufficienttofullyavoid induced platelet dysfunction.23,24 Treatment options for patients theplateletdysfunctionassociatedwithibrutinib. thatareathighriskofbleedingarecurrentlylimitedandtheclinical Ibrutinib causes platelet dysfunction downstream of the GPVI efficacyofplatelettransfusionhasnotbeenestablished.2Evidence receptor, GPIb, and integrin a b .9-11 Although XLA is not thatplatelettransfusionmayreverseplateletdysfunctioncausedby IIb 3 associatedwithincreasedriskofbleeding,deficientexpressionor ibrutinib is based on in vitro data11 with few studies investigating functionofGPVI,12-14GPIb,15orintegrina b 16isassociatedwith this approach clinically.25 Furthermore, the benefit of platelet IIb 3 bleedingphenotypesinmiceorhumans.Theprecisereasonforthe transfusion during treatment with other antiplatelet medication is 12DECEMBER2017xVOLUME1,NUMBER26 ACALABRUTINIBAVOIDSSEVEREPLATELETDYSFUNCTION 2611 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. A NR -3 p>0.05 ml) -4 g/ p>0.05 or C (M 50 -5 p>0.05 gE p>0.05 Heathy Donors nist lo -6 Ibrutinib Patient o g A -7 Acalabrutinib Patient Treatment Naive Patient -8 -9 ADP U46619 Epinephrine TRAP-6 CRP-XL Collagen B C 120 120 100 100 n n missio 80 missio 80 ns ns 60 a a ht tr 60 ht tr Healthy Donors g g 40 Max li 40 p < 0.001 Max li Acalabrutinib Patients % % 20 p < 0.001 Ibrutinib Patients 20 0 Btk Inhibitor Naive Patients 0 -20 -10 -9 -8 -7 -6 -5 -10 -9 -8 -7 -6 -5 log [CRP-XL] (g/ml) log [collagen] (g/ml) D E Acalabrutinib Ibrutinib 100 100 [Inhibitor]M 80 80 Vehicle on on 0.1 missi 60 missi 60 0.3 ns ns a a ht tr 40 ht tr 40 1 g g % li % li 3 10 20 20 0 0 -8 -7 -6 -5 -8 -7 -6 -5 log[CRP] (g/ml) log[CRP] (g/ml) Figure1.AcalabrutinibandibrutinibtherapycausedysfunctionalGPVI-mediatedplateletaggregation.PRPfrompatientsreceivingibrutinib(Ibr;n56), acalabrutinib(Acal;n57),healthydonors(n59),orBtkinhibitorna¨ıveCLLpatients(n55)wasloadedinto96-wellmicrotiterplatescontaininglyophilizedplateletagonists. Plateswereshakenfor5minutesat37°Candaggregationwasmeasurebylighttransmissiontogiveanendpointmeasurement.(A)ScatterplotofEC50valuescalculatedfrom 2612 BYEetal 12DECEMBER2017xVOLUME1,NUMBER26 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. controversial and may lead to poorer outcomes.26 Investigating centrifuging at 350g for 20 minutes and resuspending the platelet alternatives to platelet transfusion to treat or prevent bleeding pelletat43108cells/mLinTyrode’sbufferaspreviouslydescribed.9 duringibrutiniboracalabrutinibtherapyisthereforeapriority.One Plate-basedaggregometry. Formeasurementofaggrega- alternative to platelet transfusion for bleeding patients, or those tion using PRP from patients or healthy donors, 96-well plates undergoingsurgeryandatriskofbleedingfromplateletdysfunction, (Greiner)containingthefollowingfreeze-driedplateletagonistsata isadministration of desmopressin,27-29 which stimulates secretion range of concentrations: ADP, CRP-XL, epinephrine, U46619, of the contents of Weibel-Palade bodies and results in an acute collagen, and TRAP-6 were prepared in advance and stored in increase in plasma von Willebrand factor (VWF) and factor VIII vacuum-sealedbagsfornomorethan2months.PRPisolatedfrom (FVIII)levelsoftwo-tosixfold.30Indeed,successfuladministrationof thebloodofhealthydonorsorpatientswasloadedontoplatesand desmopressintostopbleedinginpatientssufferingfromthrombo- shaken at 1200 rpm for 5 minutes at 37°C using a plate shaker cytopenia has also been reported.31 It may be possible to (Quantifoil Instruments), as described by Lordkipanidze´ et al; administer desmopressin to treat bleeding or reduce bleeding risk absorptionof405nmlightwasmeasuredusingaMultiskanAscent during treatment with Btk inhibitors, either as an alternative for or 354 Microplate Reader (LabSystems). Aggregation of washed adjunct to platelet transfusion. However, because ibrutinib inhibits plateletswasperformedin96-wellplatesaspreviouslydescribed.9 GPIb-mediated platelet function,11 it has remained unclear if this approachmightbebeneficial. Thrombusformationunderflow. Thrombusformationwas performedusingbloodfromhealthydonorsusingmicrofluidicflow Methods chips (Vena8, CellixLtd, Dublin, Ireland) coated with 100 mg/mL type I collagen and measured in real time following incubation of Materials bloodfromhealthydonorswithibrutinib,acalabrutinib,orvehiclefor 10 minutes, or fixed with 10% formyl saline after 8 minutes of TypeIcollagenwasobtainedfromNycomed(Munich,Germany)and perfusionatashearrateof1000s21andimagedatalatertime. collagen-relatedpeptide(CRP-XL)fromProfessorRichardFarndale (University of Cambridge, Cambridge, United Kingdom). Adenosine Protein phosphorylation studies. Washed platelets at 59-diphosphate (ADP), arachidonic acid, and U46619 were from 4 3 108 cells per milliliter in the presence of inhibitors to prevent Sigma(Gillingham,United Kingdom), and TRAP-6 epinephrine was aggregation(100mMMRS2179,1mMcangrelor,10mMindometh- from Labmedics (Salford, United Kingdom). Acalabrutinib, ibrutinib, acin,and1mMEGTA)wereincubatedwithibrutiniboracalabrutinibat anddasatinibwerefromSelleckchem(Munich,Germany).Antiphos- concentrationsspecifiedinindividualfiguresorvehiclefor5minutesat photyrosineantibody4G10wasobtainedfromMillipore(Burlington, 37°Cbeforeadditionof1mg/mLCRP-XL.Sampleswereincubatedfor MA).PKCsubstrateantibodyandphospho-PLCg2Y759wasfrom 3minuteswithstirringat37°Cusinganaggregometer(Helena)before NewEnglandBiolabs (Hitchin,UnitedKingdom).Phospho-Src418 additionofreducingLaemmlisampletreatmentbuffer. antibodyandFura-2AMwasfromLifeTechnologies(Paisley,United Phospho-Tec ELISA. Platelets were prepared and stimu- Kingdom).Phospho-BtkY223,phospho-LynY396,andphospho-b3 latedasdetailedpreviouslybutlysedinNP40buffer(300mMNaCl, Y773 antibodies were from Abcam (Cambridge, United Kingdom). 20mMTrisbase,2mMEGTA,2mMEDTA,1mMPMSF,10mg/mL Actin11CantibodywasfromSantaCruzBiotechnology(Heidelberg, aprotinin,10mg/mLleupeptin,0.7mg/mLpepstatinA,2mMsodium Germany). Greiner 96-well plates and DiOC6 were from Thermo orthovanadate,2%v/vNP-40;pH7.3)andanalyzedusingahuman FisherScientific(Dartford,UnitedKingdom). phosphotyrosine Tec enzyme-linked immunosorbent assay (ELISA Patients. Trough blood samples were obtained from patients kit,RayBio).Absorptionat405nmwasmeasuredusingaNOVOstar withCLLormantlecellleukemiaandreceivingeitheribrutinib(6patients) platereader(BMGLabTech,Aylesbury,UnitedKingdom). oracalabrutinib(8patients;Table1).OurcontrolgroupcomprisedBkt- Ca21 measurement. The [Ca21] assay was performed at inhibitorna¨ıveCLLpatients(5patients).Allpatientsprovidedinformed i 37°Cusingfura-2loadedwashedplateletsinblack96-wellplates consentinaccordancewiththedeclarationofHelsinki.Ethicsapproval (Greiner). Dual excitation was measured using a Novostar forthisstudywascoveredundertheOxfordRadcliffeBiobankresearch spectrofluorometer(BMGLabtech)previouslydescribed.9 tissuebankethics,HTALicenseNumber12217,OxfordshireCREC: 09/H0606/515,projectapprovalcode17/A016. Platelet adhesion to collagen. Washed platelets at 23107cells/mLwereexposedtocollagen(100mg/mL)-coated, Platelet preparation. Blood samples were obtained from 96-wellassayplates,andallowedtoadherefor45minutesat37°C. healthy donors that had given informed consent and using Nonadherent platelets were washed off before, fixed with 10% proceduresapprovedbytheUniversityofReadingResearchEthics formyl saline for 10 minutes. The wells were then washed and Committeeorfrompatientsandcollectedintovacutainerscontaining labeled with DiOC6. Fluorescence images of adherent platelets 3.8%(w/v)sodiumcitrate.Platelet-richplasma(PRP)wasprepared werecapturedwiththe203objectivelensofanImageXpressNano bycentrifugingwholebloodat100gfor20minutes.Washedplatelets high content imaging system and counted using CellReporterX- were prepared by adding acid citrate dextrose to PRP and presssoftware(MolecularDevices,Winnersh,UnitedKingdom). Figure1.(continued)concentrationresponsecurvesforADP,U46619,epinephrine,TRAP-6,CRP-XL,andcollagen.Eachpointrepresentstheresponseofapatientreceiving acalabrutinib(redtriangle)oribrutinib(greensquare);healthydonor(graycircle)orBtkinhibitorna¨ıveCLLpatient(whitediamond).NR,patientsthatdidnotrespondtoanagonist atthehighestconcentrationtested.ConcentrationresponsecurvesforGPVIagonists(B)CRP-XLand(C)collagen;eachpointrepresentsthemean%aggregationvalues6 standarderrorofthemean(SEM).Significantdifferencesrelativetohealthydonorsweretestedby2-wayANOVAwiththeTurkeymultiplecomparisonstest.Aggregationofwashed plateletsfromhealthydonorspre-treatedwitharangeof(D)acalabrutinibor(E)ibrutinibconcentrationsandthenstimulatedwith3to0.01mg/mLCRP-XL. 12DECEMBER2017xVOLUME1,NUMBER26 ACALABRUTINIBAVOIDSSEVEREPLATELETDYSFUNCTION 2613 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. A B Acalabrutinib Ibrutinib 200 200 % vehicle phosphorylation 11550000 SBT(Pert)cck- Y YtYo24ta21l38 % vehicle phosphorylation 11550000 0 0 Vehicle-9 -8 -7 -6 -5 -4 Vehicle-9 -8 -7 -6 -5 -4 log[acalabrutinib] (M) log[ibrutinib] (M) log [Acalabrutinib] (M) log [Ibrutinib] (M) C V -8 -7.5 -7 -6.5 -6 -5.5 -5 V -8 -7.5 -7 -6.5 -6 -5.5 -5 Btk Y223 50 50 Src Y418 50 Actin loading control D E F G 140 140 140 140 % vehicle Lyn Y396 phosphorylation 11864220000000 % vehicle total phosphotyrosine 11864220000000 % vehicle aggregation 11864220000000 % vehicle adhesion 11864202000000 AIDbcaruastlaaintbiinbriubtinib 0 0 0 0 Vehicle-8 -7 -6 -5 Vehicle-8 -7 -6 -5 Vehicle-8 -7 -6 -5 Vehicle-8 -7 -6 -5 log[inhibitor] (M) log[inhibitor] (M) log[inhibitor] (M) log[inhibitor] (M) H log [Acalabrutinib] (M) log [Ibrutinib] (M) log [Dasatinib] (M) V-7.5-7-6.5-6-5.5-5 V-7.5-7-6.5-6-5.5-5 V-7.5-7-6.5-6-5.5-5 Lyn Y396 4G10 Total Phosphotyrosine Actin Figure2.SFKactivationandadhesiontocollagenissparedbyacalabrutinibbutnotibrutinib.Washedhumanplateletsfromhealthydonorswerepreincubated witharangeof(A)acalabrutinibor(B)ibrutinibandthenstimulatedwith1mg/mLCRP-XLfor3minutesat37°C;tyrosinephosphorylationofSrc(Y418)andBtk(Y223)were measuredbywesternblotusingsite-specificantibodiesandtotallevelsofTectyrosinephosphorylationweremeasurebyELISA.Pointsrepresentmeanlevelsoftyrosine phosphorylationrelativetovehicle-treatedcontrols6SEM.(C)Representativeimagesofphosphoblots.Washedplateletstreatedwitharangeofacalabrutinib,ibrutinib,or dasatinibconcentrationsandstimulatedaspreviouslyandblottedfor(D)tyrosinephosphorylationofLyn(Y396)or(E)totalphosphotyrosineusingasite-specificantibodyor 4G10,respectively.Pointsrepresentmeanlevelsoftyrosinephosphorylationrelativetovehicle-treatedcontrols6SEM.(F)Aggregation1mg/mlCRP-XLstimulatedofwashed plateletswasperformedin96-wellplatesaftertreatmentwitharangeofconcentrationsofacalabrutinib,ibrutinib,ordasatinibconcentrationresponsecurvesaremeanplatelet 2614 BYEetal 12DECEMBER2017xVOLUME1,NUMBER26 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. Fluorescence-activated cell sorting measurement of Acalabrutinib is selectivefor SFK but not Tec fibrinogenbindingandp-selectinexposure. Measurements of Both ibrutinib and acalabrutinib have been screened for activity fibrinogen binding and p-selectin exposure were performed againstapanelofkinasesincell-free,invitroassays.8,33However, using washed platelets pretreated with inhibitors as described the estimated potency of the drugs in such assays does not in figure legends and stimulated with 1 mg/mL CRP in the correspond closely with measurements performed in cell-based presence of fluorescein isothiocyanate–conjugated polyclonal assays. In addition to this, kinase regulation in the platelet is highly rabbit anti-fibrinogen antibody (Agilent Technologies LDA UK complexandinvolvespositiveandnegativefeedbackmechanisms.34 Limited, Cheadle, United Kingdom) and PE-Cy5-conjugated To elucidate the mechanistic differences between ibrutinib and mouseanti-P-selectin(CD62P)antibody(BD,Berkshire,United acalabrutinibthatunderpindifferencesinbleedingrisk,wecharacter- Kingdom), and then incubated for 20 minutes in the dark. izedtheeffectsofthedrugsonphosphorylationeventsdownstreamof Platelets were then fixed by addition of filtered formyl saline GPVIinplateletsfromhealthydonors (Figure2).Phosphorylation of (0.2% formaldehyde in 0.15M NaCl) and median fluorescence BtkY223,theautophosphorylationsiteofBtkthatcorrelateswithits intensitiesweremeasuredfor5000plateletspersampleonan kinaseactivity,wasinhibitedwithequalpotencybyibrutinib(loghalf AccuriC6FlowCytometer(BDBiosciences,Berkshire,United maximal inhibitory concentration [logIC ] 5 27.2M 6 0.30) and Kingdom). 50 acalabrutinib(logIC 527.1M60.21;Figure2A-B).InhibitionofTec 50 Statistical methods. Statistical testing as described in was harder to quantify because of the lack of site-specific phospho figure legends and the results section were performed using antibodies, but total phosphotyrosine levels can be measured by GraphPadPrismSoftware(GraphPad,LaJolla,CA). ELISA. Total Tec phosphotyrosine levels are likely to include the Tec autophosphorylationsiteY20635aswellastyrosineresiduesphosphor- Results ylatedbyotherkinasessuchasSFK.WeestimatedthatTecwasmore potentlyinhibitedbyibrutinib(logIC 526.4M)thanbyacalabrutinib 50 Acalabrutiniband ibrutinib cause dysfunction of (logIC 525.5M;Figure2A-B);however,theconcentration-response 50 GPVI-mediated platelet aggregation profilesofbothibrutinibandacalabrutinibwerecomplex,involvingboth positiveandnegativecomponentsanddifferentialregulationofmultiple PlateletaggregationtoGPVIagonistshaspreviouslybeenshownto sites. Phosphorylation of the autophosphorylation site Y418 of Src be inhibited in blood samples taken from patients receiving appeared to be potentiated by both drugs at lower concentrations. ibrutinib,10,11 but the effect of acalabrutinib on platelet function However, at higher concentrations, ibrutinib also inhibited Src Y418 has not been reported. Aggregation of PRP was used to phosphorylation(logIC 525.7M60.18),whereasacalabrutinibdid characterize platelet function of patients treated with ibrutinib or 50 not inhibit Src activity and actually potentiated activation even at high acalabrutinib (Table 1). One patient receiving acalabrutinib was concentrations(logEC 527.5M60.46;Figure2A-B).Becauseour excluded from this aspect of the study because of a low platelet 50 data indicated that platelet Btk and Tec were likely to be inhibited count (,50 3 109/L). The aggregation assay included ADP, by physiological concentrations of both ibrutinib and acalabrutinib, U46619, epinephrine, thrombin receptor activator peptide-6 we further investigated inhibition of SFK by comparing both drugs to (TRAP-6), CRP-XL, and collagen was adapted from the method the SFK inhibitor dasatinib. Phosphorylation of Lyn Y396 (Figure 2D) developedandvalidatedbyLordkipanidze´ etal.32Weusedarange was ablated by dasatinib (logIC 5 27.1M 6 0.05) and ibrutinib of agonist concentrations to enable comparison of patient (logEC 5 25.8M 6 0.08)5b0ut not acalabrutinib, which only sensitivity to each agonist by estimation of the log half maximal 50 inhibited phosphorylation to 70% of vehicle-treated platelets at effective concentration (logEC ) by nonlinear regression analysis. 50 the highest concentration tested (10 mM). Total phosphotyrosine Results were compared with a group of healthy donors and Btk levels(Figure2E)followedasimilarpatternwherebydasatinibcaused inhibitorna¨ıveCLL patients (Figure 1A). Aggregationstimulated by near ablation of CRP-XL–evoked tyrosine phosphorylation ADP, U46619, epinephrine, and TRAP-6 was not significantly (logIC 5 26.9M 6 0.24), whereas ibrutinib was less potent different in either patient group compared with healthy controls. (logIC505 25.1M 6 0.29) and acalabrutinib only inhibited partially Responsestocollagenwerecompletelyablatedinallpatientstested 50 (71.7%ofvehicle)at10mM. forbothpatientgroupsreceivingBtkinhibitors,evenatthehighest concentrationofcollagen(3mg/mL)(Figure1A-B).Responsestothe Ibrutinib but not acalabrutinib potently inhibits GPVI receptor agonist CRP-XL were either less potent (ibrutinib,2 platelet adhesion tocollagen patients; acalabrutinib, 3 patients) or ablated (ibrutinib, 4 patients; acalabrutinib, 4 patients) relative to responses of healthy controls Aggregationofwashedplateletsevokedby1mg/mLCRP-XLwas (logEC 5 27.7M 6 0.30; Figure 1C) and Btk inhibitor na¨ıve completelyablatedbyacalabrutinib(logIC 525.3M60.06)and 50 50 CLL patients (logEC50 5 27.3M 6 0.38). Experiments in which withsignificantlygreaterpotencybyibrutinib(logIC 526.2M6 50 CRP-XL was titrated against ibrutinib and acalabrutinib indicated 0.28)anddasatinib(logIC 526.6M60.6;Figure2F).Wehave 50 that 10mM acalabrutinib or 1mM ibrutinib was required to ablate previouslyreportedthatdiscrepancies arepresentinthewaythat platelet aggregation of washed platelets from healthy donors ibrutinib inhibits platelet aggregation to immobilized collagen- (Figure1D-E). coatedsurfaces.9Adhesionofplateletstocollagen(Figure2G)was Figure2.(continued)aggregation6SEMrelativetovehicle-treatedcontrol.(G)Acalabrutinib,ibrutinib,ordasatinib-treatedwashedplateletsfromhealthydonorswere allowedadheretocollagen-coatedwellsofa96-wellplateafter45minutesat37°C;graphsplotconcentrationresponsecurvestomeannumbersofadheredplatelets6SEM relativetovehicletreatment.(H)Representativeimagesofphosphoblotsforplateletstreatedwithtyrosinekinaseinhibitors. 12DECEMBER2017xVOLUME1,NUMBER26 ACALABRUTINIBAVOIDSSEVEREPLATELETDYSFUNCTION 2615 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. A B 140 140 120 120 PLC2 (P) Y759 18000 P) PKC substrate 18000 % vehicle 4600 % vehicle ( 4600 Ibrutinib 20 Acalabrutinib 20 0 0 Vehicle -9 -8 -7 -6 -5 -4 Vehicle -9 -8 -7 -6 -5 -4 log[inhibitor] (M) log[inhibitor] (M) C log [Acalabrutinib] (M) log [Ibrutinib] (M) V -8 -7.5 -7 -6.5 -6 -5.5 -5 V -8 -7.5 -7 -6.5 -6 -5.5 -5 PLC2 (Y759) 37 150 100 (P) S/T 75 PKC Substrates 50 37 25 20 50 D E Acalabrutinib 140 120 Vehicle 2+ [Ca] 18000 2+M [Ca]i 000...1303MMM % vehicle 60 100 n 60s 13MM 40 F Ibrutinib 10M 20 0 Vehicle -9 -8 -7 -6 -5 -4 +]i log[inhibitor] (M) 2a C M [ n 0 0 60s 1 Figure3.AcalabrutinibinhibitssignaltransductiondownstreamofGPVIwithlowerpotencythanibrutinib.Washedhumanplateletsfromhealthydonorswere preincubatedwitharangeofacalabrutiniboribrutinibconcentrationsandthenstimulatedwith1mg/mLCRP-XLfor3minutesat37°Candphosphorylationof(A)PLCg2 2616 BYEetal 12DECEMBER2017xVOLUME1,NUMBER26 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. A B C 140 140 140 120 120 120 % vehicle P-selectin exposure 186400000 % vehicle fibrinogen binding 186400000 % vehicle (P) Y7733 186400000 Acalabrutinib 20 20 20 Ibrutinib 0 0 0 Vehicle-9 -8 -7 -6 -5 -4 Vehicle-9 -8 -7 -6 -5 -4 Vehicle-9 -8 -7 -6 -5 -4 log[inhibitor] (M) log[inhibitor] (M) log[inhibitor] (M) D log [Acalabrutinib] (M) log [Ibrutinib] (M) V -8 -7.5 -7 -6.5 -6 -5.5 -5 V -8 -7.5 -7 -6.5 -6 -5.5 -5 150 - 3 Y773 100 75 50 - Actin loading control Figure4.AcalabrutinibisalesspotentinhibitorofintegrinaIIbb3activationandgranulesecretionthanibrutinib.Washedhumanplateletsfromhealthydonors werepreincubatedwitharangeofacalabrutiniboribrutinibconcentrationsandthenstimulatedwith1mg/mLCRP-XLfor20minutes.(A)P-selectinand(B)fibrinogenbinding wasmeasuredbyfluorescence-activatedcellsorting.(C)Plateletswerestimulatedwith1mg/mLCRP-XLfor3minutesat37°C.Phosphorylationofb3(Y773)was measuredbywesternblotting.Pointsrepresentmeanresponsesrelativetovehicle6SEM.(D)Representativeb3(Y773)blots. partiallyinhibited(;40%ofvehicle)byibrutinib(logIC 525.9M6 stimulated downstream of PLCg2 and was also inhibited less 50 0.18) and dasatinib (logIC 5 26.9M 6 0.09), which closely potentlybyacalabrutinib(logIC 526.1M60.08)thanibrutinib 50 50 matchedtheirabilitytoinhibitLynactivity.Acalabrutinibwasaweak (logIC 526.760.07,P,.05,Studentttest). 50 inhibitorofadhesiontocollagenandonlyreducedthenumberof adheredplateletto60%69.4ofvehicle. Acalabrutinib inhibits granule secretion and integrin a b activation less potently than ibrutinib IIb 3 Acalabrutinibinhibits signalingdownstream ofGPVI Secretionofa-granuleswasinvestigatedbymeasuringexposureof less potently than ibrutinib P-selectin on the platelet surface following stimulation with CRP- To understand the consequences of the differences in kinase XL. P-selectin exposure was more potently inhibited by ibrutinib specificity of the inhibitors, signaling events downstream of the (logIC 526.5M60.04)thanbyacalabrutinib(logIC 525.9M6 50 50 kinases were measured. We found that phosphorylation of the 0.11; Figure 4A). Binding of fluorescently labeled fibrinogen was Btk substrate, Y759 of PLCg2, was inhibited by both ibrutinib used as measure of integrin a b activation following stimulation IIb 3 (logIC 5 26.7M 6 0.18) and acalabrutinib (logIC 5 26.7 6 with CRP-XL (Figure 4B). Fibrinogen binding was inhibited more 50 50 0.26;Figure3B).However,acalabrutinibdidnotcompletelyablate potently by ibrutinib (logIC 5 26.5M 6 0.04) than by 50 phosphorylation of PLCg2 Y759 even at the highest concentra- acalabrutinib (logIC 5 25.8M 6 0.07). Phosphorylation of the 50 tionofacalabrutinibtested.PhosphorylationofPKCsubstrateswas integrinb subunitisacriticaleventintheinitiationofintegrina b 3 IIb 3 inhibitedlesspotentlybyacalabrutinib(logIC 526.2M60.19) outside-insignaling.Phosphorylationofb Y773(correspondingto 50 3 thanbyibrutinib(logIC 526.560.24,P,.05,Student ttest; Y747inmouse)waspotentlyinhibitedbybothibrutinib(logIC 5 50 50 Figure3B).AcalabrutinibinhibitedPKCactivityby52%64.5relative 26.7M 6 0.13) and acalabrutinib (logIC 5 26.6M 6 0.11. 50 tovehicle,significantlylessthanibrutinib,whichinhibitedby72%6 Figure4C).Acalabrutinibappearedtobeonlyapartialinhibitorof 3.3 (P , .05, Student t test) at the highest concentration b Y773phosphorylation,becauseevenatthehighestconcentra- 3 tested. Release of Ca21 from intracellular stores into the cytosol is tiontested,a reductiontoonly27%62.5relative tovehiclewas Figure3.(continued)(Y759)and(B)PKCsubstrates(S/T)wasmeasuredbywesternblotting.(C)RepresentativewesternblotimagesforPLCg2(Y759)andS/T phosphorylatedPKCsubstrates.(D)CytosolicCa21followingstimulationwith1mg/mLCRP-XLwasmeasuredinfura-2loadedplateletsinrealtimefor5minutes.Points representthemeanresponserelativetovehicle6SEM.Representative[Ca21]itracesfollowingincubationwith(E)acalabrutinibor(F)ibrutinib. 12DECEMBER2017xVOLUME1,NUMBER26 ACALABRUTINIBAVOIDSSEVEREPLATELETDYSFUNCTION 2617 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. Figure5.Ibrutinib,butnotacalabrutinib,causesthrombus A instability.Wholebloodfromhealthydonorswasincubatedwith vehicle,1mMibrutinib,and1mMacalabrutinibfor20minutesand e flowedthroughcollagen-coatedmicrofluidicflowchambersata hicl shearrateof1000s21for6minutes.(A)Representativeimagesof e V thrombiformedundereachoftheconditionstestedat2-minute intervals.(B)Asummaryofeffectsof1mMibrutiniband1mM acalabrutinibonthrombusformationoncollagenandotherplatelet b Mni signalingandfunctionalmeasurementsrelativetovehicle-treated 1bruti control.Barsrepresentthemean6SD;Pvalueswerecalculated I usingmultipletestswithHolm-Sidakcorrectionformultiple comparisons. b ni Muti br 1a al c A 0 2 min 4 min 6 min 8 min B 250 1M Ibrutinib p=0.054 1M Acalabrutinib onse 200 p=0.046 p=0.002 esp 150 p=0.003 p=0.002 p=0.011 hicle r 100 p=0.009 p=0.007 e % v 50 p=0.814 0 Src (Y418B)tk (Y223)Tec (P-Y) [Ca2+Fi]b binP-disnelg exposuArgegregationAdhmebsiuos nformation Thro achieved, whereas ibrutinib caused inhibition to 6% 6 1.0 of importantsignalingandfunctionalmeasurementsaresummarized vehicle. inFigure5B. To test whether experiments performed using blood from Acalabrutinibavoids dysfunctional thrombus healthy donors matched the effects of drugs at therapeutic formation caused by ibrutinib concentrations, we performed measurements of thrombus Giventhedifferencesintheeffectsofthedrugsonadhesionto formationoncollagenunderarterialshearusingbloodsamples collagen compared with GPVI-mediated aggregation, we com- from healthy donors, Btk-inhibitor na¨ıve patients, or patients paredtheeffectsofthedrugsonplateletadhesionandthrombus receiving ibrutinib or acalabrutinib (Table 1). Blood from formationincollagen-coatedflowchambersunderarterialshear acalabrutinib patients formed morphologically normal thrombi conditions. After treating whole blood from healthy donors with on collagen (Figure 6A), although heterogeneity in platelet either 1mM ibrutinib or acalabrutinib for 20 minutes, ibrutinib counts strongly influenced thrombus volume (Figure 6C). causedreducedthrombusformation(1mMibrutinib:383AU640.1, Thrombusvolumeinacalabrutinibpatientswithplateletcounts vehicle 585AU 6 67.6, P , .05, Student t test), whereas in .100 3 109/L (78895 mm3 6 16258) were not significantly thepresenceofvehicleoracalabrutinib,thrombusformationwas different to those of Btk-inhibitor na¨ıve patients (75608 mm3 6 not significantly different (Figure 5A-B). The most striking 19995, P . .05, Student t test). In contrast, thrombus volume differencebetweenibrutinibandacalabrutinibtreatmentwasthe foribrutinibpatientswashighlyvariableanddidnotcorrelatewith lack of stable, retracted thrombi after ibrutinib treatment plateletcount(Figure6D).Imagesofthrombimeasuredinsamples (Figure 5A). In the presence of vehicle or acalabrutinib, platelets from patients with platelet counts .150 3 109/L are presented in accumulated on collagen fibers while continuously contracting Figure 6A. Samples from 2 of the ibrutinib patients exhibited very into dense thrombi, whereas ibrutinib prevented retraction of pronounceddysfunctionwherebyplateletsformedaloosecovering platelet aggregates, which consequently remained unstable, ofthemajorityofthesurfaceoftheflowchamberwithoutforming appearedloose,andwerepronetodisaggregation(supplemental stable thrombi (“large”; Figure 6A), whereas others formed small Video1).Theeffectsof1mMibrutinibandacalabrutinibonseveral thrombi(“small”;Figure6A). 2618 BYEetal 12DECEMBER2017xVOLUME1,NUMBER26 From www.bloodadvances.org by guest on January 7, 2019. For personal use only. A (-) Haemate P (+) Haemate P y h alt e H b hie nv k INai Bt al c A e Ibrarg L brmall IS 400m 600m 200m 0 B C D 3m) 300000 (-) Haemate P 3m) 300k 3m) 300000    me ( 200000 (+) Haemate P non-zero slope me ( 200k non-zero slope me ( 200000 mbus volu 100000 pp==00..045609 mbus volu 100k pp==00..002461 mbus volu 100000 Thro 0 Thro 0k Thro 0 0 50 100 150 200 250 300 0 50 100 150 200 0 50 100 150 200 Platelet count (x109 / L) Platelet count (x109 / L) Platelet count (x109 / L) Figure6.Thrombusformationoncollagencorrelateswithplateletcountduringtreatmentwithacalabrutinibbutnotwithibrutinib.(A)Bloodfromhealthy donors(n56),Btk-inhibitorna¨ıveCLLpatients(n55),patientsreceivingibrutinib(n56)oracalabrutinib(n58)wasperfusedthroughcollagen-coatedmicrofluidicflow chambersatroomtemperatureatashearrateof1000s21beforebeingfixedwith10%formylsaline.FixedsampleswerestainedwithDioC6andz-stackimagesacquiredto enableestimationofthrombusvolume.(A)RepresentativeimagesofthrombiinbloodfromahealthydonorandpatientsinthepresenceorabsenceofHaemateP(intermediate factorVIII)addedexvivo.Thrombusvolumeplottedagainstplateletcountfor(B)Btkinhibitorna¨ıveCLLpatients;patientstreatedwith(C)acalabrutinibor(D)ibrutinibwithor withoutaddedHaemateP.CorrelationbetweenplateletcountandthrombusvolumeissignificantinthepresenceorabsenceofHaematePforacalabrutinibpatients (significantlynonzero,P#.05)butnonsignificantforibrutinibpatients(P..05). Addition ofHaemate Pex vivo topatients’ blood repeated measures and the Sidak multiple comparisons test; improves platelet function Figure7). Thrombus formation assays using patients’ blood were per- Discussion formedinthepresenceorabsenceof2units/mLofHaemateP. Correlation of thrombus volume with platelet count was not Ibrutinibhasproventobeaneffectivetreatmentoflow-gradeNHL significant within the Btk-inhibitor na¨ıve patient group because but is associated with an increased risk of bleeding, whereas the platelet counts were all .100 3 109/L and thrombus volume effects of the second-generation Btk inhibitor, acalabrutinib, on was fairly uniform. The correlation was significant in patients platelet signaling and function have not been studied in detail. treated with acalabrutinib in the presence and absence of Ibrutinibhasbeenshowntoinhibitplateletaggregationevokedby HaemateP(Figure6B),butnotinpatientstreatedwithibrutinib GPVIreceptoragonists,9-11buttheeffectsofacalabrutinibtherapy (Figure 6C), despite half of the patients having platelet counts on platelet aggregation have not been reported. We found that ,100 3 109/L, which strongly influences thrombus volume. aggregation evoked by collagen and CRP-XL was either partially AdditionofHaematePsignificantlyincreasedthrombusvolume or completely inhibited in all patients receiving ibrutinib or in healthy donors and patients treated with acalabrutinib or acalabrutinib (Figure 1). Peak plasma concentrations of ibrutinib ibrutinib (P , .05, 2-way analysis of variance (ANOVA) with and acalabrutinib have been estimated at approximately 300 nM 12DECEMBER2017xVOLUME1,NUMBER26 ACALABRUTINIBAVOIDSSEVEREPLATELETDYSFUNCTION 2619 From www.bloodadvances.org by guest on January 7, 2019. For personal use only.

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Alexander P. Bye,1 Amanda J. Unsworth,1 Michael J. Desborough,2,3 .. kinase activity, was inhibited with equal potency by ibrutinib (log half.
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