Incorporation Into Lipid Nanoparticles Extends the Duration of Activity of Treprostinil in an Acute Hypoxia Rat Model of Pulmonary Arterial Hypertension
D Omiatek1, F Leifer1, V Malinin1, J Ong1, T Henn1, Z Li1, RW Chapman1, D Salvail2, CE Laurent2, WR Perkins1 1Insmed, Inc., Bridgewater, NJ, USA
2IPS Therapeutique Inc., Sherbrooke, QC, Canada
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LNPs effectively retained TRE to provide sustained release
In vitro bioavailability of TRE was slowed for TRE in LNPs
Figure 4. TRE-LNP drug release screened by dialysis
LNPs, lipid nanoparticles; TRE, treprostinil.
Figure 5. TRE-LNP efficacy screened by cAMP assay on CHO-K1 cells
Concentration of cAMP data was 1 µM TRE for each sample. cAMP, cyclic adenosine monophosphate; CHO-K1, Chinese hamster ovary; LNP, lipid nanoparticle; TRE, treprostinil; TRE-LNP, treprostinil lipid nanoparticle.
In Vivo TRE-LNP Characterisation Results
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Inhaled TRE-LNPs extend vasodilatory effect as compared with TRE
Inclusion into LNP extends blood plasma levels of inhaled TRE
Figure 6. TRE-LNP efficacy screened in a rat model of pulmonary arterial hypertensionmPAP, mean pulmonary arterial pressure; PBS, phosphate-buffered saline, TRE, treprostinil; TRE-LNP, treprostinil lipid nanoparticle.
Figure 7. TRE-LNP pharmacokinetic profile in a rat model of pulmonary arterial hypertension
TRE, treprostinil; TRE-LNP, treprostinil lipid nanoparticle.
Figure 3. Manufacturing conditions of flow rate ratio (FRR) (A) and total flow rate (B) affect treprostinil–lipid nanoparticle (TRE-LNP) particle size
TREPROSTINIL
CATIONIC LIPID
PHOSPHOLIPID
HYDROPHOBICFILLER
PEGYLATEDLIPID
Figure 1. (A) Chemical structure of treprostinil (TRE) and (B) schematic representation of treprostinil lipid nanoparticles (TRE-LNPs)
INTRODUCTION• Treprostinil(TRE)isaprostacyclinanalogueusedtotreatpulmonaryarterialhypertension(PAH).• Inthisstudy,wedesignedaTREdeliverysystembasedonthedevelopmentofalipidnanoparticle(LNP)suspensionforencapsulationandsustainedreleaseofthedrug.
• Uniform,nanoscaletreprostinil–lipidnanoparticles(TRE-LNPs)(Figure 1)werecomposedof(i)TRE,(ii)acationiclipidtoamalgamatewiththelipophilicandcomplementarynegativelychargedterminusoftheTREmolecule,(iii)apolymericcoatingtostabiliseparticlesandenhancetheirbioavailability,(iv)ahydrophobic“filler”moleculetostabilisethecoreoftheparticle,and(v)anominalconcentrationofphospholipidtoaffixthepegylatedlipidtotheLNPcomposite.
AIMS• TodesignaninhalableTREformulationforthetreatmentofPAHthatwouldhaveanimprovedpharmacokinetic(PK)profilerelativetothecurrentinhaledTREtherapyforPAH,Tyvaso®,tofacilitateaonce-dailydosingschedule
–Toachievethis,wedevelopedabioavailableTREvehiclecarrierwithanoptimiseddrugpayload andreleaseprofiletosupportasustainedvasodilatoryresponserelativetofreeTRE.
Nanoparticle Formation at Miscible Fluid Interface
Lipid/ Organic Solvent Inlet
NanoparticleOutlet
1 mm
25 nm
Aqueous Solvent
Inlet
Aqueous Solvent
Inlet
Figure 2. Manufacture of treprostinil–lipid nanoparticles (TRE-LNPs) by solvent flash precipitation
METHODSTRE-LNP Production• Solventflashprecipitationviamicroscaleflowfocusingwasusedfortheone-step,continuousflowsynthesisofuniformnanoscaleTRE-LNPs(Figure 2).
• Inthisprocess,acenterstreamofalcohol-solvatedTREandlipidisimpingedwithaqueousstreamspositionedperpendiculartotheTREstream.
–Astheaqueousstreamsmeetwithandlaterallyfocusthemiscible-solvatedlipidstream,theorganicandaqueousphasesinterdiffuse,producingasolventcompositioninwhichthelipidsareincreasinglylesssoluble.
–Thiscausesthelipidstoself-associateintointermediateassembliesthateventuallycloseonthemselvesintosphericalnanoscaleLNPs.
In Vitro TRE-LNP Characterisation Methods • Releasekineticsscreenedbydialysis –50kDamolecularweightcutoffforcelluloseacetatemembrane –InitialconcentrationofTREwas100μM –1mLofsamplewasdialysedagainst1Lof1xphosphate-bufferedsaline(PBS)for24hours.
• Efficacyscreenedinamammaliancellassay(foracompletedescriptionofthesemethods,seeposterbyChenK-J,etal,ERSPoster#2358)
–Chinesehamsterovary(CHO-K1)cells(ATCC®CCL-61)weretransientlyco-transfectedwiththepGloSensorTM-22FcAMPplasmid(PromegaCorporation,Madison,WI)andtheprostanoidreceptorEP2-plasmid.
–TransfectedcellswerethentreatedwithTREanddifferentformulationsofTRE-LNPs. –Cyclicadenosinemonophosphate(cAMP)levelsweremeasuredevery5minutesforthedura-
tionofthestudies,andtheincreaseinactivationrelativetothecontrolsampleswascalculated.
LNP Size Controlled Via Process Variables• Bycontrollingtheflowrateratio(FRR)oftheaqueous:alcohol-solvateddrugstreamsandthetotal flowrateofthesystem,theTRE-LNPparticlesizecanbefine-tuned(Figure 3). –Particlesizeisknowntoplayaroleinformulationbioavailability.
In Vivo TRE-LNP Characterisation Methods• RatmodelofPAH –MaleSpragueDawleyratswereanaesthetised,artificiallyventilatedandpreparedformeasure-
mentofmeanpulmonaryarterialpressure(mPAP),meansystemicbloodpressure(mSAP),heartrate(HR),andarterialoxygensaturation(SaO2).
–Physiologicparametersweremeasuredduringnormoxia(fractionofinspiredoxygen[FiO2]=0.21,SaO2≈90%)andfor2to3hoursduringhypoxia(FiO2=0.10,SaO2≈50%).
–BloodsamplesweretakenovertimeandlungtissueharvestedattheendofthestudytomeasureTREconcentration(HPLC/MS/MSanalysis).
–CompoundsweredeliveredviaAeroneb®(Aerogen,Galway,Ireland)nebuliserinterposedinaventilatorcircuit(seeposterbyMalininetal,ERSPoster#2367)atanestimatedpulmonarydoseaof2µg/kg.
aMeasuredfromTREconcentrationinlungimmediatelypostdose.
RESULTSIn Vitro TRE-LNP Characterisation Results
CONCLUSIONS• Inthepresentstudy,wesoughttodevelopaninhaledTRE-LNPformulationforthetreatmentofPAHtoimprovethedurationofthetherapeuticbenefitandthetolerabilityofTRE.OptimisationofTRE-LNPformulationwasbasedonparticlesizeandTREreleasekinetics.ActivitywasassessedinvitroinCHO-K1cellsusingapGloSensorassayandinvivoinanacutehypoxiaratmodelofPAH.
• AgradualincreaseincAMPactivationofCHO-K1cellssuggestedaslowed-releaseprofileoftheTREnanoparticleformulationrelativetothefreedrug.
• Inthehypoxicratmodel,thepulmonaryvasodilatoryactivityofinhaledTRE-containingLNPswasextendedbeyondthatofinhaledTREinsolution,whichisconsistentwithanextendedPKprofileofthedrugobservedinexcisedbloodplasma.
• PackagingTREintoananoparticleformulationincreaseddurationofthevasodilatoryeffectrelativetothefreedrug,butisunlikelytofacilitateaonce-dailydosingschedulebasedonthepharmacokineticprofileobserved.
• TofurtherimprovenanoparticleretentionofTRE,wedevelopedaderivatisedTREprodrugmadebycovalentattachmentofalkylchains(seeposterbyLeiferetal,ERSPoster#2356).WebelievethatthisapproachwillresultinasustainedvasodilatoryresponsewellbeyondthatobservedwithTRE-LNPsandfreedrug.
Please see other posters in this series:• Leifer F, et al, ERS Poster #2356 • Chen K-J, et al, ERS Poster #2358 • Malinin V, et al, ERS Poster #2367
ACKNOWLEDGEMENTSTheauthorswouldliketoacknowledgeConnexionHealthcare(Newtown,PA)forprovidingeditorial,layout,anddesignsupport.Insmed,Inc.(Bridgewater,NJ)providedfundingtoConnexionHealthcarefortheseservices.
Poster presented at the European Respiratory Society (ERS) International Congress, 6-10 September, 2014, Munich, Germany.
Table 1. TRE-LNP Formulation Characteristics
Formulation
Mole Percent of TRE-LNP
Particle Size (nm)TRE Cationic Lipid
Hydrophobic Filler Phospholipid
Pegylated Lipid
TRE-LNP-1 15 30 35 0 10 47
TRE-LNP-2 5 15 60 10 10 59
TRE-LNP-3 2 10 68 10 10 45
TRE TRE-LNPsA B
TRE-LNP, treprostinil lipid nanoparticle.
A BPa
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ize
(nm
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Part
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Siz
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FRR Aqueous:Drug/Lipid Streams Total Flow Rate (mL/min)
POSTER #: 2357
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