WO2020160087A1 - Methods of separating long polynucleotides from a composition - Google Patents

Methods of separating long polynucleotides from a composition Download PDF

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Publication number
WO2020160087A1
WO2020160087A1 PCT/US2020/015577 US2020015577W WO2020160087A1 WO 2020160087 A1 WO2020160087 A1 WO 2020160087A1 US 2020015577 W US2020015577 W US 2020015577W WO 2020160087 A1 WO2020160087 A1 WO 2020160087A1
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Prior art keywords
composition
polynucleotides
pores
long
kilobase
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French (fr)
Inventor
Jennifer Louise SCHMITKE
Robert John Lyng
Vishwesh Ashok PATIL
Can SARISOZEN
Marcus Ian GIBSON
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Flagship Pioneering Innovations V Inc
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Flagship Pioneering Innovations V Inc
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Priority to US17/425,545 priority Critical patent/US20220098574A1/en
Priority to EP20747950.2A priority patent/EP3918065A4/en
Publication of WO2020160087A1 publication Critical patent/WO2020160087A1/en
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/10Processes for the isolation, preparation or purification of DNA or RNA
    • C12N15/1003Extracting or separating nucleic acids from biological samples, e.g. pure separation or isolation methods; Conditions, buffers or apparatuses therefor
    • C12N15/1017Extracting or separating nucleic acids from biological samples, e.g. pure separation or isolation methods; Conditions, buffers or apparatuses therefor by filtration, e.g. using filters, frits, membranes
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D61/00Processes of separation using semi-permeable membranes, e.g. dialysis, osmosis or ultrafiltration; Apparatus, accessories or auxiliary operations specially adapted therefor
    • B01D61/14Ultrafiltration; Microfiltration
    • B01D61/145Ultrafiltration
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D61/00Processes of separation using semi-permeable membranes, e.g. dialysis, osmosis or ultrafiltration; Apparatus, accessories or auxiliary operations specially adapted therefor
    • B01D61/14Ultrafiltration; Microfiltration
    • B01D61/18Apparatus therefor
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D61/00Processes of separation using semi-permeable membranes, e.g. dialysis, osmosis or ultrafiltration; Apparatus, accessories or auxiliary operations specially adapted therefor
    • B01D61/14Ultrafiltration; Microfiltration
    • B01D61/22Controlling or regulating
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D2311/00Details relating to membrane separation process operations and control
    • B01D2311/14Pressure control
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D2313/00Details relating to membrane modules or apparatus
    • B01D2313/20Specific housing
    • B01D2313/203Open housings
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D2313/00Details relating to membrane modules or apparatus
    • B01D2313/24Specific pressurizing or depressurizing means

Definitions

  • the present invention includes methods of separating long polynucleotides from a composition.
  • One aspect of the invention provides a method of separating long polynucleotides from a composition.
  • the method includes: introducing a composition including one or more long polynucleotides into a container including at least one boundary defined by a filter comprising a plurality of pores, wherein the pores have a smaller cross-sectional dimension than specified for the long polynucleotide’s molecular weight; and applying elevated hydraulic pressure to the composition, thereby causing at least some of the one or more long polynucleotides to pass through the pores.
  • Another aspect of the invention provides a method of separating a long polynucleotide from a composition.
  • the method includes: (a) providing a composition comprising a long polynucleotide, (b) disposing the composition within a container including at. least one boundary comprising a plurality of pores having a smaller cross-sectional dimension than specified for a molecular weight of the long polynucleotide; and (c) subjecting the composition to elevated hydraulic pressure within the container under conditions to cause the long polynucleotide to pass through the pores, thereby separating the long polynucleotide from the composition.
  • the long polynucleotides can have a length of about 1 kilobase or greater.
  • the long polynucleotides can have a length selected from the group consisting of: >950 kilobase, >900 kilobase, >850 kilobase, >800 kilobase,
  • the composition further can include a second component.
  • the second component may not pass through the pores.
  • the filter can be positioned within the container between an inlet and an outlet and the composition can be flowed over the filter.
  • the composition can be flowed laterally over the filter
  • the elevated hydraulic pressure can be between about 0.1 and about 30 pounds per square inch (psi), inclusive.
  • the elevated hydraulic pressure can be below/ a pressure that would impact the stability of other components of the composition
  • the long polynucleotides can be sheared during passage through the pores.
  • the pores can have an effective molecular weight cutoff of about 1,000 kDa.
  • the pores can have a maximum cross-sectional dimension between about 50 run and about 150 nm.
  • FIG. 1 depicts tangential flow filtration according to an embodiment of the invention.
  • FIG. 2 depicts of generalized proportions of long polynucleotides (e.g., messenger RNA) and Hpid-based nanopartieles (LNPs).
  • long polynucleotides e.g., messenger RNA
  • LNPs Hpid-based nanopartieles
  • FIG. 3 depicts the passing of long polynucleotides through the pores of a filter while long polynucleotides encapsulated within LNPs are retained according to embodiments of the invention.
  • FIG. 4 depicts mRNA concentrations in the retentate vs. wash cycles.
  • FIG. 5 depicts encapsulation efficiency (EE) and recovery for different lipid-based nanoparticles (LNPs) encapsulating different cargos.
  • LNP_3, LNP_5 and LNP_1 1 were loaded with sgRNA (100 nt, -34 kDa).
  • the LNP+mRNA formulation contained mRNA
  • FIG. 6 depicts EE and recovery values of an optimized LNP formulation encapsulating rnRNA, processed by an embodiment of the invention.
  • the present invention is directed to, among other things, methods of purifying polynucleotides or other components from a mixture by tangential flow filtration.
  • lipid nanoparticle comprising at least one rnRNA
  • boundary refers to an edge that defines an extent past which a substance (e.g., long polynucleotides within a composition) cannot pass, at least without a reduction in concentration or physical deformation.
  • a boundary may exist within a container such that the boundary limits passage from a first chamber to a second chamber.
  • a boundary may also exist on an external surface such that boundary limits flow of a substance into or out of the container ’ fire boundary may be in-line with a direction of flow of the composition or may be lateral to a direction of flow.
  • exemplary containers refers to any receptacle that holds a substance such as a fluid or liquid.
  • exemplary containers can be finite such as a bucket, a syringe, and the like.
  • Exemplary containers can also be continuous such as cylinders, tubing, and the like that can have arbitrary lengths.
  • cross-sectional dimension refers to the largest dimension transverse to a longest axis.
  • cross-sectional dimension of a rectangular cuboid having a length of 10, a width of 4, and a height of 3 would have a eross-sectional dimension of 5 (the diagonal of the width -by -height).
  • hydroaulic pressure as used herein is defined as force applied by a liquid over a unit area.
  • nucleic acids are polymers of nucleotides.
  • nucleic acids and polynucleotides as used herein are interchangeable.
  • pore refers to an opening in a filter through with a filtrate can pass through, but which retains (at least in part) a retentate.
  • the present invention includes methods of purifying free polynucleotides from other components, where either the polynucleotides or the other components are suitable for administration as a pharmaceutical product based on tangential How filtratio (TFF).
  • the mixture comprises polynucleotides and proteins.
  • the mixture comprises non-protein components, such as nanoparticles, and polynucleotides.
  • the mixture comprises any combination of components and polynucleotides.
  • PBS polynucleotide
  • polynucleotides are present (-4500 kDa), this method cannot he used because the largest molecular weight cutoff for dialysis membranes is 300 kDa, far smaller tha the polynucleotides. While high pressures might push long polynucleotides through the 300 kDa membrane, the pressure levels required for effective purification will negatively impact nanoparticle stability and cause nanoparticle breakdown during the membrane pass. Furthermore, the removal process takes significantly longer time, generally requiring 24- 8h of dialysis.
  • the second method involves using centrifugal ultrafil ration devices.
  • the nanoparticles are pushed through a membrane by applying extreme g-force. But if the g-force is too low, the removal of free polynucleotides is limited. If the force is high, then stability of the nanoparticles is negatively affected, e.g., the nanoparticles are crushed.
  • the present invention is, in part, based on the discovery that tangential flow filtration is surprisingly effective to remove components, e.g., byproducts, in particular, guide RNAs or other free polynucleotides, from polynucleotide mixtures.
  • tangential flow filtration can effectively remove components, e.g., byproducts such as gRNA or other free polynucleotides, while still maintaining the integrity of polynucleotides or the other component.
  • the present invention includes a more effective, reliable, and safer method of purifying KNA, assembled nanoparticles, or other components from large scale manufacturing and processing of therapeutics.
  • Lipid-based nanoparticies are one of the most effective non-viral transfection strategies for in vivo delivery of nucleic acid-based therapeutics, including RNA-based therapeutics.
  • LNPs are typically composed of four main lipid types: a cationic or ioniieree lipid, a neutral helper lipid, cholesterol for structural integrity, and steriealiy stabilizing lipid.
  • Cationic an ioniieree lipids contain a functional group (e.g., an amine group) that carries a permanent positive charge or that can be positively charged at low pH values and, thus, complex the negatively charged RNA (e.g., mRNA) and different guide RNAs (dual or single).
  • Steriealiy stabilizing lipids are usually PEG-lipid conjugates (e.g., PEG-DMG), which cover the surface of the LNPs and shield overall surface charges (positive or negative), making the surface hydrophilic.
  • PEG-lipid conjugates e.g., PEG-DMG
  • PEG-DMG PEG-lipid conjugates
  • In vivo applications of steriealiy stabilizing lipids prevent opsonization and increase the longevity of the LNPs in the blood.
  • the present invention includes a process of encapsulating messenger RNA (mRNA) in lipid nanoparticies by methods known to those of skill in the art, such as by mixing a mRNA solution and a lipid solution.
  • mRNA messenger RNA
  • RNA molecules are important because free (or naked) RNA molecules would have a significantly shorter half-life in the blood circulation (usually measurable in minutes). Moreover, non-encapsulated mRNA molecules that are not effectively removed from drug products may he immunogenic.
  • mRN mRN
  • removal of free/non-encapsulated nucleic acids, e.g., free guide RNAs, mRNAs, etc., and purification of LNPs are equally important as encapsulating the mRN As (e.g., those having greater than about 1,400 bases, about 1,350 bases, about 1,300 bases, about 1,250 bases, about 1 ,200 bases, about 1,150 bases, about 1,100 bases, about 1,050 bases, about 1,000 bases, about 950 bases, about 900 bases, about 850 bases, about 800 bases, about 750 bases, about 700 bases, about 650 bases, about 600 bases, and the li See).
  • mRN e.g., those having greater than about 1,400 bases, about 1,350 bases, about 1,300 bases, about 1,250 bases, about 1 ,200 bases, about 1,150 bases, about 1,100 bases, about 1,050 bases, about 1,000 bases, about 950 bases, about 900 bases, about 850 bases, about 800 bases, about 750 bases, about 700 bases,
  • the present invention includes a composition comprising LNPs associated with at least one mRNA (e g., greater than about 1,400 bps, about 1,350 bps, about 1,300 bps, about 1,250 bps, about 1,200 bps, about 1,150 bps, about 1,100 bps, about 1,050 bps, about 1,000 bps, about 950 bps, about 900 bps, about 850 bps, about 800 bps, about 750 bps, about 700 bps, about 650 bps, about 600 bps, and the like) and one guide RNA (e.g., less than 100 bps) (e.g., LNP+mRNA+gRNA is an assembled LNP), wherein greater than about 90% of the LNPs have an individual particle size of less than about 100 mrt (e.g., less than about 95 nm, about 90 nm, about 85 nm, about 80 nm, about 75 nm, about 70 mn, about 65 nm, about 60 mRNA (e.g.,
  • substantially all of the LNPs have an individual particle size of less than about 100 nm (e.g., less than about 95 nm, about 90 nrn, about 85 nm, about 80 nm, about 75 n , about 70 nm, about 65 nm, about 60 nm, about 55 nm, or about 50 nm). In some embodiments, greater than about 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98%, or 99% of the assembled LNPs encapsulate at least one mRNA within each individual particle. In some embodiments, substantially all of the LNPs encapsulate at least one mRNA and/or at least one guide RNA within each individual particle.
  • a composition according to the present invention includes at least about 1 mg, 5 mg, 10 mg, 100 g, 500 g, or 1000 mg of encapsulated mR A and/or guide RNA.
  • some of the LNPs will not include a payload, will not include gRNA, will not include mRNA, will only include gRNA, will only include mRNA, and the like.
  • Embodiments of the invention exploit the physical characteristics of polynucleotides such as RNA relative to other components, e.g., lipid-based nanoparticles (LNPs).
  • LNPs lipid-based nanoparticles
  • Applicant believes that long polynucleotides are relatively narrow and have high aspect ratios. For example, polynucleotides are believed to have a maximum cross-sectional width of about 3 nm regardless of length, which can be on the order of about 300 nm for about a 1,000 base pair polynucleotide. These proportions of long polynucleotides 202 are depicted conceptually in FIG. 2.
  • the polynucleotides behave in ways that are unexpected based on conventional filtration techniques that are based on the molecular weight of components of a feed. For example and as depicted conceptually in FIG. 3, the long
  • polynucleotides 202 can pass through a filter 306 having pores 308 that are smaller than specified for molecules having the long polynucleotide’s molecular weight. Without being bound by any particular theory, Applicant believes that this is attributable to the narrow' cross- sectional dimension of the long polynucleotides 202 relative to the larger cross-sectional dimension of LNPs 204 encapsulating the long polynucleotides 202.
  • the invention includes a method of separating polynucleotides from a composition (e.g., purifying mRNA from a LNP).
  • separating polynucleotides comprises separating short polynucleotides (e.g., less than 100 bps in length) as well as separating long polynucleotides (e.g., greater than 1,000 bps in length).
  • the long polynucleotides e.g., greater than 1,000 bps in length.
  • the long polynucleotides e.g., greater than 1,000 bps in length.
  • polynucleotide has a length of 1 kb (kilobases) or greater. Although filtration of long polynucleotides 1s unexpected, embodiments of the invention capable of separating long polynucleotides would also be able to separate short polynucleotides.
  • the pore-containing filter is at an end of a container and fluid i pressed against the filter (e.g., by gravity or other pressure source).
  • the filter is a tangential flow filtration device in which the filter is positioned laterally to the feed flow direction. Such a device is depicted in FIG. 1.
  • Tangential flow filtration also referred to as cross-flow filtration, is a type of filtration wherein the material to be Altered is passed tangentially across a filter rather than through it.
  • TFF In TFF, undesired permeate passes through the filter, while the desired retentate passes along the filter and is collected downstream. It is important to note that the desired material is typically contained in the retentate in TFT, which is the opposite of what one normally encounters in traditional-dead end filtration.
  • Tangential- or cross-flow filters can have a variety of architectures including hollow fiber, spiral wound, and flat plate. Suitable filters are available from a variety of sources including: Cole-Parmer of Vernon Hills, Illinois, Mill t pore Corporation of Billerica,
  • TFF is usually used for either microfiltration or ultraf itration .
  • Microfiltration is typically defined as instances where the filter has a pore size of
  • NMWL nominal molecular weight limits
  • MWCO molecular weight cut off
  • Tangential-flow filtration can be implemented on industrial scale and can include system(s) adapted, configured, and/or programmed to periodically take steps to delay or prevent fouling of the filter.
  • the system can backwash the filter by periodically inverting the transmembrane pressure (TMP), providing alternating tangential flow, cleaning-in-place with detergents, reactive agents, and alkalis, and periodically closing or reducing flow from the permeate outlet.
  • TMP transmembrane pressure
  • transmembrane pressure is the force that drives fluid through the filter, carrying with it permeable molecules.
  • the transmembrane pressure is between about 0.5 and about 10 pounds per square inch (psi), inclusive.
  • Elevated pressure can be measured across the filter.
  • the elevated pressure can be a pressure gradient generated in-whole or in-part by a vacuum on the opposite side from the composition or a back-pressure valve on the retentate.
  • elevated pressure can be generated by fluid flow velocity, syringes, pumps (e.g., peristaltic pumps), and the like.
  • the elevated pressure can be a pressure gradient between about 0.5 and about 10 pounds per square inch (psi) (between about 3,500 and about 70,000 Pascal).
  • Shear rate is the rate at which a progressive shearing deformation is applied to some material.
  • Exemplar ⁇ ' shear rates are between about 1,000 and about 2.0,000 s "1 (e.g,
  • the feed rate (also known as the crossflow velocity) is the rate of the solution flow' through the feed channel and across the filter.
  • the feed rate determines the force that sweeps away molecules that may otherwise clog or foul the filter and thereby restrict filtrate flow.
  • the feed rate is between about 50 and about 500 mL/minute. In some embodiments, the feed rate is between about 50 and about 400 mL/minute. In some
  • the feed rate is between about 50 and about 300 mL/minute. In some embodiments, the feed rate is between about 50 and about 300 mL/minute.
  • the feed rate is between about 50 and about 200 mL/minute. In some embodiments, the feed rate is between about 50 and about 200 mL/minute.
  • the feed rate is between about 75 and about 200 mL/minute. In some embodiments, the feed rate is between about 75 and about 200 mL/minute.
  • the feed rate is between about 100 and about 200 mL/minute. In some embodiments, the feed rate is between about 100 and about 200 mL/minute.
  • the feed rate is between about 125 and about 175 mL/minute. In some embodiments, the feed rate is between about 125 and about 175 mL/minute. In some embodiments, the feed rate is between about 125 and about 175 mL/minute.
  • the feed rate is about 130 mL/minute. In some embodiments, the feed rate is between about 60 mL/min and about 220 mL/min. In some embodiments, the feed rate is about 60 mL/min or greater. In some embodiments, the feed rate is about 100 mL/min or greater. In some embodiments, the feed rate is about 150 mL/min or greater. In some embodiments, the feed rate is about 200 mL/min or greater. In some embodiments, the feed rate is
  • the tangential flow filtration is performed at a feed rate of approximately 100-200 mL/minute (e.g., approximately 100-180 mL/minute. 100-160 mL/minute, 100-140 mL/minute, 110-190 mL/minute, 110-170 mL/minute,
  • the tangential flow filtration is performed at a feed rate of
  • the flow rate of the permeate is the rate at which the permeate is removed from the system.
  • increasing permeate flow rates can increase the pressure across the filter, leading to enhanced filtration rates while also potentially increasing the risk of filter clogging or fouling.
  • the principles, theory, and devices used for TFT are described in Michaels et ah, "Tangential Flow Filtration" in Separations Technology, Pharmaceutical and
  • HP-TFF high-performance tangential flow filtration
  • the flow rate is between 10 and 100 mL/minute. In some embodiments, the flow rate is between about 10 and about 90 mL/minute. In some embodiments, the flow rale is between about 10 and about 80 ml, /minute. In some embodiments, the flow rate is between about 10 and about 70 mL/minute. In some embodiments, the flow rate is between about 10 and about 60 mL/minute. In some embodiments, the flow rate is between about 10 and about 50 mL/minute. In some embodiments, the flow rate is between about 10 and
  • the flow rate is between about 20 and
  • the flow rate is about 30 mL/minute.
  • flow rates to accommodate large (commercial) scale purification entail the tangential flow filtration is performed at a feed rate of approximately 10-200 L/minute. (e.g., approximately 10-180 L/minute, 100-160 L/minute, 100-140 L/minute, 1 10-190 L/minute,
  • the tangential flow filtration is performed at a feed rate of
  • Flux is a measure of the magnitude of flow across the membrane. Exemplary flux values are between about 20 and about 200 (e.g °.. betwee about 25 and about 55 -- ).
  • a filter can include a plurality of pores. Pores can have a regular, uniform shape such as a cylindrical or a rectangular profile, and the like, or cart have an irregular profile. The pores can have a nanoseale and may not be capable of dimensional measurement. Instead, the pores may be measured based on filtration performance, e.g. , based o what molecular weight particles will and/or will not pass through the filter.
  • the term‘"molecular weight cut-off ' or MWCO refers to the lowest molecular weight solute (in dal tons) in which x% (typically 90) of the solute is retained by a membrane.
  • filters used in the invention described herein may have any of a variety of pore sizes. Pore size determines the nominal molecular weight limits (NMWL), also referred to as the molecular weight cut off (MWCO) for a particular fi lter, with mierofiltration membranes typically having NMWLs of greater than about 1,000 kilodaltons (kDa) and ultrafiltration filters having NMWLs of between about 1 kDa and about 1,000 kDa
  • NMWL nominal molecular weight limits
  • MWCO molecular weight cut off
  • a filter will have a NMWL of between about 100 kDa and about 1 ,500 kDa. In some embodiments, a filter will have a NMWL. of between about 500 kDa and about 1,000 kDa. In some embodiments, a filter will have a NMWL between about 600 kDa and about BOOkDa. In some embodiments, a filter has a NMWL of about 750 kDa.
  • filters having an MWCO of about 1,000 kDa and/or a maximum cross-sectional dimension between about 100 nm and about 150 n are particularly advantageous for filtering long polynucleotides. This is significantly lower than the 1,500 kDa molecular weight of 4,500 kbp mRNA.
  • the maximum cross-sectional dimension of the filter is about, 99, 100, 110, 120, 130, 140, or 150 nm, and any and all values in between or has a MWCO of about 700, 750, 800, 850, 900, 950, 1000, 1050, and any and all values in between.
  • This Example demonstrates mRNA synthesis.
  • mRN A is typically thought of as the type of RNA that carries information from DNA to the ribosome.
  • the existence of mRNA is typically very brief and includes processing and translation, followed by degradation.
  • large scale quantities of mRNA may- need to he purified away from IVT ⁇ in vitro synthesis) components.
  • purified RNA may further be utilized in subsequent preparations, e.g., polynucleotide loaded nanoparticles.
  • mRN A is synthesized.
  • IVT is typically performed with a linear or circular DNA template containing a promoter, a pool of ribonucleotide triphosphates, a buffer system that may include DTT and magnesium ions, and an appropriate RNA polymerase (e.g., T3, T7 or SP6 RNA polymerase), DNAse I, pyrophosphatase, and/or RNAse inhibitor.
  • a promoter e.g., a promoter
  • a buffer system e.g., DTT and magnesium ions
  • an appropriate RNA polymerase e.g., T3, T7 or SP6 RNA polymerase
  • mRNA is synthesized via in-vitro transcription from a linearized DNA template.
  • IVT mRNA precursor
  • a mixture of 100 p.g of linearized DNA, rNTPs (3 33 ruM), DTT (10 raM), T7 RNA polymerase, RNAse Inhibitor, Pyrophosphatase and reaction buffer (10x, 8Q0mM Hepes (pH8.0), 20mM Spermidine, 250 niM MgC12, pH 7 7) is prepared with RNase-free water to a final volume of 2.24 ml..
  • the reaction mixture is incubated at 37°C for a range of time between 20 minutes and 120 minutes. Upon completion, the mixture is treated with DNase I for an additional 15 minutes and quenched accordingly.
  • the IVT mRNA is diluted in 4x volume of PBS pH 7.4 immediately after quenching.
  • This Example demonstrates preparation of a protein and polynucleotide mixture.
  • RNA and protein are present in whole cell lysates, nuclear, and/or cytoplasmic fractions. Isolation of large scale, high quality RNA is becoming more popular. In some circumstances, complementary proteins from the same preparations are also required. Usually these preparations are performed using different separation protocols, wasting large quantities of the preparation to purify one component. The addition of independent preparations and separation protocols is costly and time-consuming.
  • the following Example demonstrates preparation of a protein and polynucleotide mixture for separation.
  • 'Tissue or cultured cells are homogenized in ice-cold Ceil Disruption Buffer (2M KC1, 1 M MgCl?, 1M pH 7.5 Tris-Cl, RNase-free 3 ⁇ 40) to prepare a total cell lysate. Homogenization is performed quickly on ice and in the presence of detergent (1M DTT). The lysate is diluted in 4x volume of PBS pH 7.4 immediately after homogenization.
  • Lipid-based nanoparticles are an effective delivery vehicle for in-vivo deliver ' of nucleic acid-based therapeutics, including RNA-based ones.
  • Sterically stabilizing lipids may include PEG- lipid conjugates (i.e. PEG-DMG), which cover the surface of the LNPs and shield overall surface charges (positive or negative), make the surface hydrophilic, and in in vivo applications, prevent opsonization to increase longevity in the blood.
  • PEG-DMG PEG- lipid conjugates
  • the LNP formulations were prepared by mixing a lipid ethanol solution (organic phase) with mRNA (large mRNA with 4500 kb, molecular weight is approx. 1500 kDa) having a pH 4.5 in an aqueous buffer (aqueous phase) at predetermined aqueous-to-organi c phase volume ratios of 2: 1 or 3: 1 and flow rates varying from 2 mi/miii to 8 ml/min in a microfiuidies-hased preparation chip. (Ratios between about 1 : 1 and about 4: 1 and/or flow rates between
  • the resulting LNP dispersion included ethanol, whose percentage was dependent on the mixing ratio.
  • This Example demonstrates separatio of polynucleotides from other components in a mixture.
  • Purification methods are typically based on the removal of polynucleotides through filtration with membranes having MWCO sizes of at least 1500 kDa for 4500kb length polynucleotides.
  • High MWCO membranes such as 1000 kDa, have pore sizes as big as 100 nm, thus other components leak out from the membrane, causing material loss and impure separations.
  • he second method involves using centrifugal u 1 trail 1 trail on devices.
  • the mixture components are pushed through a membrane by applying extreme g-force. But if the g ⁇ force is too low, the removal of free polynucleotides is limited. If the force is high, then stability 7 of the components is negatively affected, i.e., the components are crushed. Moreover, the solution that contains the ra NA and products to be purified wi ll be stationary ' at the membrane contact surface, which can cause clogging of the pores in such membranes.
  • the ethanol removal ami buffer exchange are performed on a tangential flow filtration (TFF) device with a molecular weight cut off (MWCO) of 750 kDa.
  • TCF tangential flow filtration
  • MWCO molecular weight cut off
  • Example 1 The final products of Example 1 or Example 2 may be used as a substitute to the LNP dispersion of Example 3 in the following.
  • Example 3 The LNPs dispersion of Example 3 was concentrated to 1 ml volume (initial volume depends on the batch size, usually between 12-100 ml after mixing in PBS). Then the separation of polynucleotides from LNPs w 7 as performed by washing the mixtures three times with PBS, each time with 10 ml volume. Each time, the mixtures were concentrated to 1 ml volume.
  • the buffer exchange/purification/concentration was achieved by passing the mixture through the TFF device by applying pressure, either manually via syringes or automatically via a system equipped with pumps (e g., peristaltic pumps) and pressure sensors, in the distal ends of the device.
  • a portion of the dispersion phase (aqueous phase) leaked out through the hollow fibers, carrying the non-encapsul ted tnRNA molecules with it (FIG. 1).
  • the transmembrane pressure exerted did not produce damage to the membrane, kept the LNP structure intact, and was in the range of about 0 to 30 psi (about 0 to 205,000 Pascal).
  • the final volume of concentrated LNPs was 0.5 ml .
  • the TFF membrane selected had a MWCO size of 750 kDa- . half the size that would be predicted for 4500kb mRNA and free rnRNA molecules of this size to stay inside the membrane.
  • the selected pressure range pushed the mRNAs through pores half the size expected for their molecular weight.
  • the relationship between the applied pressure and the MWCO size can be applied to all the previous preparations for TTF-based polynucleotide purification methods.
  • LNPs encapsulating rnRNA were prepared as described in Example 3. They were subjected to the purification process as described in Example 4 prior to characterization.
  • FIG. 4 shows the washing/removal efficacy of the 1 500 kDa mRN A as a function of washing volume/cycie number.
  • the first pass from the TFF membrane reduced the rnRNA concentration in the retentate 5-times.
  • the PBS volume to wash the mRNA solution was 5 ml .
  • the remaining mRNA in the retentate dropped to negligible amounts and 4 wash cycles (20 ml total) completely removed the mRNA.
  • Table 1 also summarizes the mRNA concentrations in the retentate.
  • the LNPs were buffered/purified/concentrated and the EE and recover) 7 wrnre determined.
  • the encapsulation efficiency and the total recovery of the mRNA was determined by a fluorescent RNA quantification assay (Life Technologies) according to the manufacturer's instructions. Briefly, aliquots ofLNP solution were diluted 1 : ! in TE buffer (measuring the non-encapsuiated free tnRNA) or 1 : 1 in TE buffer containing 2% Triton X-100 (measuring total mRNA, both encapsulated and non-encapsuiated). Assay reagent was added to each sample and fluorescent signal was quantified.
  • FIGS. 3 and 4 how ' that the method purified the LNPs encapsulated sgRNA or mRNA regardless of high or low recovery values (FIG. 3). Changing the formulation parameters, such as lipid compositions, flow rates, and mixing ratio of aqueou .organic phases allowed higher recover/ rates with higher EE values, indicating removal of free non-encapsuiated mRNA (FIG. 4).
  • [OOSSf Particle sizes of the LNPs were measured using dynamic light scattering (DLS ). Briefly, the formulations were diluted in an isotonic buffer with the same ionic equivalence and pH value as the LNP dispersion at ratios varying from 1 :20 to 1:1000 v/v. The sample was injected into the sample cell of the instrument. Following temperature equilibration for 120 seconds
  • purified polynucleotides are collected and the purified
  • polynucleotides are analyzed for impurities.
  • purified polynucleotides in the preparations of Example 1 or Example 2 and pressure filtered as described in Example 4 may be analyzed as in the following Example.
  • Coomassie-stained protein gels may be performed to determine the presence of residual proteins present before and after purifications.
  • BCA assays may be performed as well.
  • mRNA size and integrity 7 may be assessed via gel electrophoresis. Either 1.0% agarose gel or Invitrogen E-Gel precast 1.2% agarose gels may be employed. mRNA is loaded at 1.0- 1.5 pg quantities per well. Upon completion, messenger RNA bands are visualized using ethidium bromide.
  • control iuciferase mRN A may be performed using HEK293T ceils. Transfections of l gg of each mRNA construct are performed in separate wells using a lipid based-transfection reagent according to manufacturer’s protocol. Cells are harvested at selected time points (e.g., 4 hour, 8 hour, etc.) and respective protein production is analyzed. For FFL mRNA, cell lysates are analyzed for Iuciferase production via bio luminescence assays. [00931 ⁇ Examples measuring a control fluorescent RNA, a bioluminescence assay may be conducted using a Promega Luciferase Assay System (Item # El 500). The Luciferase Assay Reagent is prepared by adding Luciferase Assay Buffer to Luciferase Assay Substrate and mixing via a vortex.

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Abstract

One aspect of the invention provides a method of separating long polynucleotides from a composition. The method includes: introducing a composition including one or more long polynucleotides into a container including at least one boundary defined by a filter comprising a plurality of pores, wherein the pores have a smaller cross-sectional dimension than specified for the long polynucleotide's molecular weight; and applying elevated hydraulic pressure to the composition, thereby causing at least some of the one or more long polynucleotides to pass through the pores.

Description

METHODS OF SEPARATING LONG POLYNUCLEOTIDES FROM A COMPOSITION
CROSS-REFERENCE TO RELATED APPLICATION
[00011 This application claims the benefit of priority to U.S. Provisional Patent Application Serial No. 62/798,038, filed January 29, 2019. The entire content of this application is hereby incorporated by reference herein.
BACKGROUND OF THE INVENTION
[0002] As the fields of biologies and gene editing develop into the clinical therapies, purity of the therapeutic grows in importance.
SUMMARY OF THE INVENTION
[0003] The present invention includes methods of separating long polynucleotides from a composition.
[0004] One aspect of the invention provides a method of separating long polynucleotides from a composition. The method includes: introducing a composition including one or more long polynucleotides into a container including at least one boundary defined by a filter comprising a plurality of pores, wherein the pores have a smaller cross-sectional dimension than specified for the long polynucleotide’s molecular weight; and applying elevated hydraulic pressure to the composition, thereby causing at least some of the one or more long polynucleotides to pass through the pores.
[0005] Another aspect of the invention provides a method of separating a long polynucleotide from a composition. The method includes: (a) providing a composition comprising a long polynucleotide, (b) disposing the composition within a container including at. least one boundary comprising a plurality of pores having a smaller cross-sectional dimension than specified for a molecular weight of the long polynucleotide; and (c) subjecting the composition to elevated hydraulic pressure within the container under conditions to cause the long polynucleotide to pass through the pores, thereby separating the long polynucleotide from the composition.
[0006] These aspects can have a variety of embodiments. The long polynucleotides can have a length of about 1 kilobase or greater. The long polynucleotides can have a length selected from the group consisting of: >950 kilobase, >900 kilobase, >850 kilobase, >800 kilobase,
>750 kilobase, >700 kilobase, >650 kilobase, and >600 kilobase. [0007| The composition further can include a second component. The second component may not pass through the pores.
[0008] The filter can be positioned within the container between an inlet and an outlet and the composition can be flowed over the filter. The composition can be flowed laterally over the filter
[00091 The elevated hydraulic pressure can be between about 0.1 and about 30 pounds per square inch (psi), inclusive. The elevated hydraulic pressure can be below/ a pressure that would impact the stability of other components of the composition
[0010] The long polynucleotides can be sheared during passage through the pores.
[0011[ The pores can have an effective molecular weight cutoff of about 1,000 kDa.
[0G12J The pores can have a maximum cross-sectional dimension between about 50 run and about 150 nm.
BRIEF DESCRIPTION OF THE DRAWINGS
[0013] The following detailed description of specific embodiments of the invention will be better understood when read in conjunction with the appended drawings. For the purpose of illustrating the invention, there are shown in the drawings exemplary embodiments. It should be understood, however, that the invention is not limited to the precise arrangements and
instrumentalities of the embodiments shown in the drawings.
[0014] FIG. 1 depicts tangential flow filtration according to an embodiment of the invention.
[0015] FIG. 2 depicts of generalized proportions of long polynucleotides (e.g., messenger RNA) and Hpid-based nanopartieles (LNPs).
[0016] FIG. 3 depicts the passing of long polynucleotides through the pores of a filter while long polynucleotides encapsulated within LNPs are retained according to embodiments of the invention.
[0017] FIG. 4 depicts mRNA concentrations in the retentate vs. wash cycles.
[0G18| FIG. 5 depicts encapsulation efficiency (EE) and recovery for different lipid-based nanoparticles (LNPs) encapsulating different cargos. LNP_3, LNP_5 and LNP_1 1 were loaded with sgRNA (100 nt, -34 kDa). The LNP+mRNA formulation contained mRNA
with 1 ,500 kDa size and 4500 kb. [00191 FIG. 6 depicts EE and recovery values of an optimized LNP formulation encapsulating rnRNA, processed by an embodiment of the invention.
DETAILED DESCRIPTION
[0020] In one aspect, the present invention is directed to, among other things, methods of purifying polynucleotides or other components from a mixture by tangential flow filtration.
Definitions
[00211 Unless defined otherwise, ail technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which the invention pertains. Although any methods and materials similar or equivalent to those described herein can be used in the practice for testing of the present invention, the preferred materials and methods are described herein. In describing and claiming the present invention, the following
terminology will be used.
[00221 It is also to be understood that the terminology used herein is for the purpose of describing particular embodiments only, and is not intended to be limiting.
[00231 The term '‘assembled LNP” or‘assembled lipid nanoparticle” are used interchangeable and as used herein refer to a lipid nanoparticle comprising at least one rnRNA
[00241 The term‘boundary” as used herein refers to an edge that defines an extent past which a substance (e.g., long polynucleotides within a composition) cannot pass, at least without a reduction in concentration or physical deformation. A boundary may exist within a container such that the boundary limits passage from a first chamber to a second chamber. A boundary may also exist on an external surface such that boundary limits flow of a substance into or out of the container fire boundary may be in-line with a direction of flow of the composition or may be lateral to a direction of flow.
[00251 The term“container” as used herein refers to any receptacle that holds a substance such as a fluid or liquid. Exemplary containers can be finite such as a bucket, a syringe, and the like. Exemplary containers can also be continuous such as cylinders, tubing, and the like that can have arbitrary lengths.
[0G26| The term“cross-sectional dimension”' as used herein refers to the largest dimension transverse to a longest axis. For example, the cross-sectional dimension of a rectangular cuboid having a length of 10, a width of 4, and a height of 3 would have a eross-sectional dimension of 5 (the diagonal of the width -by -height).
[0027] The term“hydraulic pressure” as used herein is defined as force applied by a liquid over a unit area.
[0028] The term“long polynucleotide” as used herein is defined as a chain of nucleotides having a length of 1000 nucleotides or more. Furthermore, nucleic acids are polymers of nucleotides. Thus, nucleic acids and polynucleotides as used herein are interchangeable.
[0029] The term“pore” as used herein refers to an opening in a filter through with a filtrate can pass through, but which retains (at least in part) a retentate.
Mixtures Containing Polynucleotides
[0030] The present invention includes methods of purifying free polynucleotides from other components, where either the polynucleotides or the other components are suitable for administration as a pharmaceutical product based on tangential How filtratio (TFF). In some embodiments, the mixture comprises polynucleotides and proteins. In some embodiments, the mixture comprises non-protein components, such as nanoparticles, and polynucleotides. In some embodiments, the mixture comprises any combination of components and polynucleotides.
[0031] Prior to the present invention, two main buffer exchange/purification/concentration methods are used in the technique of processing polynucleotide mixtures comprising
formulations. The first involves the dialysis of the polynucleotide mixtures against PBS for buffer exchange and removal of ethanol from the dispersion. However, when long
polynucleotides are present (-4500 kDa), this method cannot he used because the largest molecular weight cutoff for dialysis membranes is 300 kDa, far smaller tha the polynucleotides. While high pressures might push long polynucleotides through the 300 kDa membrane, the pressure levels required for effective purification will negatively impact nanoparticle stability and cause nanoparticle breakdown during the membrane pass. Furthermore, the removal process takes significantly longer time, generally requiring 24- 8h of dialysis.
[0032] The second method involves using centrifugal ultrafil ration devices. In this method, the nanoparticles are pushed through a membrane by applying extreme g-force. But if the g-force is too low, the removal of free polynucleotides is limited. If the force is high, then stability of the nanoparticles is negatively affected, e.g., the nanoparticles are crushed. [00331 The present invention is, in part, based on the discovery that tangential flow filtration is surprisingly effective to remove components, e.g., byproducts, in particular, guide RNAs or other free polynucleotides, from polynucleotide mixtures. As described herein, tangential flow filtration can effectively remove components, e.g., byproducts such as gRNA or other free polynucleotides, while still maintaining the integrity of polynucleotides or the other component. Thus, the present invention includes a more effective, reliable, and safer method of purifying KNA, assembled nanoparticles, or other components from large scale manufacturing and processing of therapeutics.
LNPs
[0034] Lipid-based nanoparticies (LNPs) are one of the most effective non-viral transfection strategies for in vivo delivery of nucleic acid-based therapeutics, including RNA-based therapeutics. LNPs are typically composed of four main lipid types: a cationic or ionizahle lipid, a neutral helper lipid, cholesterol for structural integrity, and steriealiy stabilizing lipid. Cationic an ionizahle lipids contain a functional group (e.g., an amine group) that carries a permanent positive charge or that can be positively charged at low pH values and, thus, complex the negatively charged RNA (e.g., mRNA) and different guide RNAs (dual or single). Steriealiy stabilizing lipids are usually PEG-lipid conjugates (e.g., PEG-DMG), which cover the surface of the LNPs and shield overall surface charges (positive or negative), making the surface hydrophilic. In vivo applications of steriealiy stabilizing lipids prevent opsonization and increase the longevity of the LNPs in the blood.
[0035] In some embodiments, the present invention includes a process of encapsulating messenger RNA (mRNA) in lipid nanoparticies by methods known to those of skill in the art, such as by mixing a mRNA solution and a lipid solution. For example, see US20180263918.
[0036] Effective encapsulation of the nucleic acids is important because free (or naked) RNA molecules would have a significantly shorter half-life in the blood circulation (usually measurable in minutes). Moreover, non-encapsulated mRNA molecules that are not effectively removed from drug products may he immunogenic. Thus, removal of free/non-encapsulated nucleic acids, e.g., free guide RNAs, mRNAs, etc., and purification of LNPs are equally important as encapsulating the mRN As (e.g., those having greater than about 1,400 bases, about 1,350 bases, about 1,300 bases, about 1,250 bases, about 1 ,200 bases, about 1,150 bases, about 1,100 bases, about 1,050 bases, about 1,000 bases, about 950 bases, about 900 bases, about 850 bases, about 800 bases, about 750 bases, about 700 bases, about 650 bases, about 600 bases, and the li See).
[0037] In some embodiments, the present invention includes a composition comprising LNPs associated with at least one mRNA (e g., greater than about 1,400 bps, about 1,350 bps, about 1,300 bps, about 1,250 bps, about 1,200 bps, about 1,150 bps, about 1,100 bps, about 1,050 bps, about 1,000 bps, about 950 bps, about 900 bps, about 850 bps, about 800 bps, about 750 bps, about 700 bps, about 650 bps, about 600 bps, and the like) and one guide RNA (e.g., less than 100 bps) (e.g., LNP+mRNA+gRNA is an assembled LNP), wherein greater than about 90% of the LNPs have an individual particle size of less than about 100 mrt (e.g., less than about 95 nm, about 90 nm, about 85 nm, about 80 nm, about 75 nm, about 70 mn, about 65 nm, about 60 nm, about 55 nm, or about 50 nm) and greater than about 70% of the LNPs encapsulate at least one mRNA and/or at least one guide RNA within each individual particle. In some embodiments, greater than about 95%, 96%, 97%, 98%, or 99% of the LNPs ha ve an individual particle size of less than about 100 nm (e.g., less than about 95 nm, about 90 nm, about 85 nm, about 80 nm, about 75 nm, about 70 nm, about 65 nm, about 60 nm, about 55 nm, or about 50 nm). In some embodiments, substantially all of the LNPs have an individual particle size of less than about 100 nm (e.g., less than about 95 nm, about 90 nrn, about 85 nm, about 80 nm, about 75 n , about 70 nm, about 65 nm, about 60 nm, about 55 nm, or about 50 nm). In some embodiments, greater than about 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98%, or 99% of the assembled LNPs encapsulate at least one mRNA within each individual particle. In some embodiments, substantially all of the LNPs encapsulate at least one mRNA and/or at least one guide RNA within each individual particle. In some embodiments, a composition according to the present invention includes at least about 1 mg, 5 mg, 10 mg, 100 g, 500 g, or 1000 mg of encapsulated mR A and/or guide RNA. In some embodiments, some of the LNPs will not include a payload, will not include gRNA, will not include mRNA, will only include gRNA, will only include mRNA, and the like.
Physical Characteristics of Polynucleotides
[0038] Embodiments of the invention exploit the physical characteristics of polynucleotides such as RNA relative to other components, e.g., lipid-based nanoparticles (LNPs). [00391 Without being hound by theory, Applicant believes that long polynucleotides are relatively narrow and have high aspect ratios. For example, polynucleotides are believed to have a maximum cross-sectional width of about 3 nm regardless of length, which can be on the order of about 300 nm for about a 1,000 base pair polynucleotide. These proportions of long polynucleotides 202 are depicted conceptually in FIG. 2.
[0040 S Due to the aspect ratio of polynucleotides, the polynucleotides behave in ways that are unexpected based on conventional filtration techniques that are based on the molecular weight of components of a feed. For example and as depicted conceptually in FIG. 3, the long
polynucleotides 202 can pass through a filter 306 having pores 308 that are smaller than specified for molecules having the long polynucleotide’s molecular weight. Without being bound by any particular theory, Applicant believes that this is attributable to the narrow' cross- sectional dimension of the long polynucleotides 202 relative to the larger cross-sectional dimension of LNPs 204 encapsulating the long polynucleotides 202.
[O041J The invention includes a method of separating polynucleotides from a composition (e.g., purifying mRNA from a LNP). In some embodiments, separating polynucleotides comprises separating short polynucleotides (e.g., less than 100 bps in length) as well as separating long polynucleotides (e.g., greater than 1,000 bps in length). In one embodiment, the long
polynucleotide has a length of 1 kb (kilobases) or greater. Although filtration of long polynucleotides 1s unexpected, embodiments of the invention capable of separating long polynucleotides would also be able to separate short polynucleotides.
TFF
[0042J A variety of filtering architectures can be utilized. In some embodiments (colloquially known as“dead-end filtration’), the pore-containing filter is at an end of a container and fluid i pressed against the filter (e.g., by gravity or other pressure source). In other embodiments, the filter is a tangential flow filtration device in which the filter is positioned laterally to the feed flow direction. Such a device is depicted in FIG. 1. Tangential flow filtration (TFF), also referred to as cross-flow filtration, is a type of filtration wherein the material to be Altered is passed tangentially across a filter rather than through it. In TFF, undesired permeate passes through the filter, while the desired retentate passes along the filter and is collected downstream. It is important to note that the desired material is typically contained in the retentate in TFT, which is the opposite of what one normally encounters in traditional-dead end filtration.
[0043] Tangential- or cross-flow filters can have a variety of architectures including hollow fiber, spiral wound, and flat plate. Suitable filters are available from a variety of sources including: Cole-Parmer of Vernon Hills, Illinois, Mill t pore Corporation of Billerica,
Massachusetts; and Repligen Corporation of Waltham, Massachusetts. Depending upon the material to be filtered, TFF is usually used for either microfiltration or ultraf itration .
Microfiltration is typically defined as instances where the filter has a pore size of
between 0.05 pm and 1.0 pm, inclusive, while ultrafiltration typically involves filters with a pore size of less than 0.05 pm. Pore size also determines the nominal molecular weight limits (NMWL). also referred to as the molecular weight cut off (MWCO) for a particular filter, with microfiltration membranes typically having NMWLs of greater than 1 ,000 kilodaltons (kDa) and ultrafiltration filters having NMWLs of between about I kDa and about 1,000 kDa.
[0044] Tangential-flow filtration can be implemented on industrial scale and can include system(s) adapted, configured, and/or programmed to periodically take steps to delay or prevent fouling of the filter. For example, the system can backwash the filter by periodically inverting the transmembrane pressure (TMP), providing alternating tangential flow, cleaning-in-place with detergents, reactive agents, and alkalis, and periodically closing or reducing flow from the permeate outlet.
[0045] A variety of filtration systems, methods, and parameters are described in Herb Lutz, Uitrafdtration for Bioprocessing: Development and Implementation of Robust Processing
(2015).
[0046] One or more process variables can be important in the TFF process: transmembrane pressure, feed rate, flow rate or flux of the permeate. The transmembrane pressure is the force that drives fluid through the filter, carrying with it permeable molecules. In some embodiments, the transmembrane pressure is between about 0.5 and about 10 pounds per square inch (psi), inclusive.
[0047] Elevated pressure can be measured across the filter. Thus, the elevated pressure can be a pressure gradient generated in-whole or in-part by a vacuum on the opposite side from the composition or a back-pressure valve on the retentate. For example, elevated pressure can be generated by fluid flow velocity, syringes, pumps (e.g., peristaltic pumps), and the like. [0G4S| The elevated pressure can be a pressure gradient between about 0.5 and about 10 pounds per square inch (psi) (between about 3,500 and about 70,000 Pascal).
[0049] Shear rate is the rate at which a progressive shearing deformation is applied to some material. Exemplar}' shear rates are between about 1,000 and about 2.0,000 s"1 (e.g,
about 7,000 s 1).
[GGS0] The feed rate (also known as the crossflow velocity) is the rate of the solution flow' through the feed channel and across the filter. The feed rate determines the force that sweeps away molecules that may otherwise clog or foul the filter and thereby restrict filtrate flow. In some embodimen s, the feed rate is between about 50 and about 500 mL/minute. In some embodiments, the feed rate is between about 50 and about 400 mL/minute. In some
embodiments, the feed rate is between about 50 and about 300 mL/minute. In some
embodiments, the feed rate is between about 50 and about 200 mL/minute. In some
embodiments, the feed rate is between about 75 and about 200 mL/minute. In some
embodiments, the feed rate is between about 100 and about 200 mL/minute. In some
embodiments, the feed rate is between about 125 and about 175 mL/minute. In some
embodiments, the feed rate is about 130 mL/minute. In some embodiments, the feed rate is between about 60 mL/min and about 220 mL/min. In some embodiments, the feed rate is about 60 mL/min or greater. In some embodiments, the feed rate is about 100 mL/min or greater. In some embodiments, the feed rate is about 150 mL/min or greater. In some embodiments, the feed rate is about 200 mL/min or greater. In some embodiments, the feed rate is
about 220 mL/min or greater.
[0051] In some embodiments, the tangential flow filtration is performed at a feed rate of approximately 100-200 mL/minute (e.g., approximately 100-180 mL/minute. 100-160 mL/minute, 100-140 mL/minute, 110-190 mL/minute, 110-170 mL/minute,
or 110-150 mL/minute) and/or a flow rate of approximately 10-50 mL/minute (e.g.,
approximately 10-40 mL/minute, 10-30 mL/minute, 20-50 mL/minute, or 20-40 mL/minute). In some embodiments, the tangential flow filtration is performed at a feed rate of
approximately 100, 110, 120, 130, 140, 150, 160, 170, 180, 190, or 200 mL/minute and/or a flow rate of approximately 10, 20, 30, 40, or 50 mL/minute.
[0052] The flow rate of the permeate is the rate at which the permeate is removed from the system. For a constant feed rate, increasing permeate flow rates can increase the pressure across the filter, leading to enhanced filtration rates while also potentially increasing the risk of filter clogging or fouling. The principles, theory, and devices used for TFT are described in Michaels et ah, "Tangential Flow Filtration" in Separations Technology, Pharmaceutical and
Biotechnology Applications (W. P. Olson, ed., Interpharm Press, Inc., Buffalo Grove, i l l .
1995). See also U.S. Pat. Nos. 5,256,294 and 5,490,937 for a description of high-performance tangential flow filtration (HP-TFF), which represents an improvement to TFF.
[0053J In some embodiments, the flow rate is between 10 and 100 mL/minute. In some embodiments, the flow rate is between about 10 and about 90 mL/minute. In some embodiments, the flow rale is between about 10 and about 80 ml, /minute. In some embodiments, the flow rate is between about 10 and about 70 mL/minute. In some embodiments, the flow rate is between about 10 and about 60 mL/minute. In some embodiments, the flow rate is between about 10 and about 50 mL/minute. In some embodiments, the flow rate is between about 10 and
about 40 mL/minute. In some embodiments, the flow rate is between about 20 and
about 40 mL/minute. In some embodiments, the flow rate is about 30 mL/minute.
[00541 A1 some embodiments, flow rates to accommodate large (commercial) scale purification entail the tangential flow filtration is performed at a feed rate of approximately 10-200 L/minute. (e.g., approximately 10-180 L/minute, 100-160 L/minute, 100-140 L/minute, 1 10-190 L/minute,
110-170 L/minute, or 1 10-150 L/minute) and/or a flow rate of approximately 10-50 L/minute (e.g., approximately 10-40 L/minute, 10-30 L/minute, 20-50 L/minute, or 20-40 L/minute). In some embodiments, the tangential flow filtration is performed at a feed rate of
approximately 100, 1 10, 120, 130, 140, 150, 160, 170, 180, 190, or 200 L/minute and/or a flow rate of approximately 10, 20, 30, 40, or 50 L/minute.
[00551 Flux is a measure of the magnitude of flow across the membrane. Exemplary flux values are between about 20 and about 200 (e.g °.. betwee about 25 and about 55 -- ).
n-nti -m '
Pores
[0056] A filter can include a plurality of pores. Pores can have a regular, uniform shape such as a cylindrical or a rectangular profile, and the like, or cart have an irregular profile. The pores can have a nanoseale and may not be capable of dimensional measurement. Instead, the pores may be measured based on filtration performance, e.g. , based o what molecular weight particles will and/or will not pass through the filter. [0057] The term‘"molecular weight cut-off' or MWCO refers to the lowest molecular weight solute (in dal tons) in which x% (typically 90) of the solute is retained by a membrane. As described herein, filters used in the invention described herein may have any of a variety of pore sizes. Pore size determines the nominal molecular weight limits (NMWL), also referred to as the molecular weight cut off (MWCO) for a particular fi lter, with mierofiltration membranes typically having NMWLs of greater than about 1,000 kilodaltons (kDa) and ultrafiltration filters having NMWLs of between about 1 kDa and about 1,000 kDa
[0058] In some embodiments, a filter will have a NMWL of between about 100 kDa and about 1 ,500 kDa. In some embodiments, a filter will have a NMWL. of between about 500 kDa and about 1,000 kDa. In some embodiments, a filter will have a NMWL between about 600 kDa and about BOOkDa. In some embodiments, a filter has a NMWL of about 750 kDa.
[0059] Without being bound by theory, Applicant believes that filters having an MWCO of about 1,000 kDa and/or a maximum cross-sectional dimension between about 100 nm and about 150 n are particularly advantageous for filtering long polynucleotides. This is significantly lower than the 1,500 kDa molecular weight of 4,500 kbp mRNA. In certain embodiments, the maximum cross-sectional dimension of the filter is about, 99, 100, 110, 120, 130, 140, or 150 nm, and any and all values in between or has a MWCO of about 700, 750, 800, 850, 900, 950, 1000, 1050, and any and all values in between.
EXAMPLES
Example 1: Synthesis of mRNA
[0060] This Example demonstrates mRNA synthesis.
[0061] mRN A is typically thought of as the type of RNA that carries information from DNA to the ribosome. The existence of mRNA is typically very brief and includes processing and translation, followed by degradation. In some embodiments, large scale quantities of mRNA may- need to he purified away from IVT {in vitro synthesis) components. In some embodiments, purified RNA may further be utilized in subsequent preparations, e.g., polynucleotide loaded nanoparticles. In the following Example, mRN A is synthesized.
[00621 Briefly, IVT is typically performed with a linear or circular DNA template containing a promoter, a pool of ribonucleotide triphosphates, a buffer system that may include DTT and magnesium ions, and an appropriate RNA polymerase (e.g., T3, T7 or SP6 RNA polymerase), DNAse I, pyrophosphatase, and/or RNAse inhibitor. The exact conditions will vary according to the specific application. The presence of these reagents is undesirable in the final product and may thus be referred to as impurities.
[00631 In the following example, mRNA is synthesized via in-vitro transcription from a linearized DNA template. To produce the desired mRNA precursor (IVT) construct, a mixture of 100 p.g of linearized DNA, rNTPs (3 33 ruM), DTT (10 raM), T7 RNA polymerase, RNAse Inhibitor, Pyrophosphatase and reaction buffer (10x, 8Q0mM Hepes (pH8.0), 20mM Spermidine, 250 niM MgC12, pH 7 7) is prepared with RNase-free water to a final volume of 2.24 ml.. The reaction mixture is incubated at 37°C for a range of time between 20 minutes and 120 minutes. Upon completion, the mixture is treated with DNase I for an additional 15 minutes and quenched accordingly.
[0064] The IVT mRNA is diluted in 4x volume of PBS pH 7.4 immediately after quenching.
Example 2: Preparation of Protein/Polynucleotide Mixtures
[0065] This Example demonstrates preparation of a protein and polynucleotide mixture.
[00661 RNA and protein are present in whole cell lysates, nuclear, and/or cytoplasmic fractions. Isolation of large scale, high quality RNA is becoming more popular. In some circumstances, complementary proteins from the same preparations are also required. Usually these preparations are performed using different separation protocols, wasting large quantities of the preparation to purify one component. The addition of independent preparations and separation protocols is costly and time-consuming. The following Example demonstrates preparation of a protein and polynucleotide mixture for separation.
[0067] 'Tissue or cultured cells are homogenized in ice-cold Ceil Disruption Buffer (2M KC1, 1 M MgCl?, 1M pH 7.5 Tris-Cl, RNase-free ¾0) to prepare a total cell lysate. Homogenization is performed quickly on ice and in the presence of detergent (1M DTT). The lysate is diluted in 4x volume of PBS pH 7.4 immediately after homogenization.
Example 3: Preparation of Polynucleotide Loaded Nanoparticles
100681 This Example demonstrates preparation of lipid-based nanoparticles (LNPs). [00691 Lipid-based nanoparticles (LNPs) are an effective delivery vehicle for in-vivo deliver ' of nucleic acid-based therapeutics, including RNA-based ones. Sterically stabilizing lipids may include PEG- lipid conjugates (i.e. PEG-DMG), which cover the surface of the LNPs and shield overall surface charges (positive or negative), make the surface hydrophilic, and in in vivo applications, prevent opsonization to increase longevity in the blood.
[0070! Effective encapsulation of nucleic adds is important since free (or naked) RNA molecules have significantly shorter half-time in the blood circulation-usually measurable in minutes. Thus, removal of free/non-encapsulated nucleic acids and purification processes of LNPs are important for effective drug delivery' of mRNAs (e.g., those having >1000 bases).
[0071! The LNP formulations were prepared by mixing a lipid ethanol solution (organic phase) with mRNA (large mRNA with 4500 kb, molecular weight is approx. 1500 kDa) having a pH 4.5 in an aqueous buffer (aqueous phase) at predetermined aqueous-to-organi c phase volume ratios of 2: 1 or 3: 1 and flow rates varying from 2 mi/miii to 8 ml/min in a microfiuidies-hased preparation chip. (Ratios between about 1 : 1 and about 4: 1 and/or flow rates between
about 1 ml/min to about 12 ml/min are also possible.) The resulting LNP dispersion included ethanol, whose percentage was dependent on the mixing ratio.
[0072J lire LNP dispersion was diluted in 10 volume of PBS pH 7.4 immediately upon collection.
Example 4: Pressure Filtration of Polynucleotide Mixtures
[0073] This Example demonstrates separatio of polynucleotides from other components in a mixture.
[0074J Purification methods are typically based on the removal of polynucleotides through filtration with membranes having MWCO sizes of at least 1500 kDa for 4500kb length polynucleotides. High MWCO membranes, such as 1000 kDa, have pore sizes as big as 100 nm, thus other components leak out from the membrane, causing material loss and impure separations.
[0075] Currently, two main buffer exchange/purification/concentration methods are used in the technique of processing mixtures with polynucleotides. The first involves the dialysis of the mixtures against PBS for buffer exchange and removal of ethanol from the dispersion. However, when large polynucleotides are present (-41500 kDa), this method cannot be used since the largest MWCO for dialysis membranes is 300 kDa, far smaller than the polynucleotides. While high pressures applied in closed-chamber systems might push large polynucleotides through the 300 kDa membrane, the pressure levels required for effective purification wi ll negatively impact stability of additional preparations in the mixture that are the main products to be purified, such as but not limited to proteins and/or LNPs, and cause potential breakdown when passing through the membrane. Furthermore, the removal process takes significantly longer time, generally requiring 24~48h of dialysis.
[00761 he second method involves using centrifugal u 1 trail 1 trail on devices. In this method, the mixture components are pushed through a membrane by applying extreme g-force. But if the g~ force is too low, the removal of free polynucleotides is limited. If the force is high, then stability7 of the components is negatively affected, i.e., the components are crushed. Moreover, the solution that contains the ra NA and products to be purified wi ll be stationary' at the membrane contact surface, which can cause clogging of the pores in such membranes. The following Example demonstrates a purification method with a membrane having a MWCO size selected to allow7 the non-encapsulated polynucleotides to be separated while keeping the other components inside the membrane. The ethanol removal ami buffer exchange are performed on a tangential flow filtration (TFF) device with a molecular weight cut off (MWCO) of 750 kDa. Moreover, the method allows the buffer exchange/putifi ca ti on/ concert trati on steps to be combined in one method and device.
[0G77f The final products of Example 1 or Example 2 may be used as a substitute to the LNP dispersion of Example 3 in the following.
[0078] The LNPs dispersion of Example 3 was concentrated to 1 ml volume (initial volume depends on the batch size, usually between 12-100 ml after mixing in PBS). Then the separation of polynucleotides from LNPs w7as performed by washing the mixtures three times with PBS, each time with 10 ml volume. Each time, the mixtures were concentrated to 1 ml volume.
[0079] The buffer exchange/purification/concentration was achieved by passing the mixture through the TFF device by applying pressure, either manually via syringes or automatically via a system equipped with pumps (e g., peristaltic pumps) and pressure sensors, in the distal ends of the device. During each pass in the membrane, a portion of the dispersion phase (aqueous phase) leaked out through the hollow fibers, carrying the non-encapsul ted tnRNA molecules with it (FIG. 1). The transmembrane pressure exerted did not produce damage to the membrane, kept the LNP structure intact, and was in the range of about 0 to 30 psi (about 0 to 205,000 Pascal). The final volume of concentrated LNPs was 0.5 ml .
[0080] The TFF membrane selected had a MWCO size of 750 kDa- . half the size that would be predicted for 4500kb mRNA and free rnRNA molecules of this size to stay inside the membrane. However, the selected pressure range pushed the mRNAs through pores half the size expected for their molecular weight. Moreover, the relationship between the applied pressure and the MWCO size can be applied to all the previous preparations for TTF-based polynucleotide purification methods.
Example 5: Characterization of LNPs
[0081] This Example demonstrates characterization of lipid-based nanoparticles (LNPs).
[0082] LNPs encapsulating rnRNA were prepared as described in Example 3. They were subjected to the purification process as described in Example 4 prior to characterization.
[0083] FIG. 4 shows the washing/removal efficacy of the 1 500 kDa mRN A as a function of washing volume/cycie number. As show in the graph, the first pass from the TFF membrane reduced the rnRNA concentration in the retentate 5-times. The PBS volume to wash the mRNA solution was 5 ml . After 3 washes (15 ml), the remaining mRNA in the retentate dropped to negligible amounts and 4 wash cycles (20 ml total) completely removed the mRNA. Table 1 also summarizes the mRNA concentrations in the retentate.
Figure imgf000017_0001
[0084] Following validation of the protocol, the LNPs were buffered/purified/concentrated and the EE and recover)7 wrnre determined. The encapsulation efficiency and the total recovery of the mRNA was determined by a fluorescent RNA quantification assay (Life Technologies) according to the manufacturer's instructions. Briefly, aliquots ofLNP solution were diluted 1 : ! in TE buffer (measuring the non-encapsuiated free tnRNA) or 1 : 1 in TE buffer containing 2% Triton X-100 (measuring total mRNA, both encapsulated and non-encapsuiated). Assay reagent was added to each sample and fluorescent signal was quantified. mRNA concentration was calculated using a calibration curve prepared with known concentrations of mRNA. The assay measured the non-encapsuiated or LNP surface bound mRNAs in the TE-diluted samples. TE- Triton X-100 (a strong detergent) broke the LNPs apart and released the encapsulated mRNA from the LNPs, thus the measured mRNA concentration was the total RNA in the LNP sample. FIGS. 3 and 4 how' that the method purified the LNPs encapsulated sgRNA or mRNA regardless of high or low recovery values (FIG. 3). Changing the formulation parameters, such as lipid compositions, flow rates, and mixing ratio of aqueou .organic phases allowed higher recover/ rates with higher EE values, indicating removal of free non-encapsuiated mRNA (FIG. 4).
[OOSSf Particle sizes of the LNPs were measured using dynamic light scattering (DLS ). Briefly, the formulations were diluted in an isotonic buffer with the same ionic equivalence and pH value as the LNP dispersion at ratios varying from 1 :20 to 1:1000 v/v. The sample was injected into the sample cell of the instrument. Following temperature equilibration for 120 seconds
backscattered light from the 488 nm laser was collected. The average particle size and polydispersity values of minimum three acquisitions were reported for each LNP formulation.
[0086] Regardless of the formulation and preparation parameters, LNP purification to remove non-encapsuiated mRNA impacted encapsulation efficiency and recovery .
[0087] The following data show that at low TMP and at high IMP, there is less efficient removal of unencapsulated mRNA relative to an intermediate TMP. This is likely due to achieving a balance between the pressure required to force tnRNAs through the pores and preventing membrane fouling at higher pressures.
Figure imgf000019_0001
Example 6: Analysis of Purified Polynucleotide
[0088] This Example demonstrates analysis of the polynucleotides separated from the other components.
[0089] In some embodiments, purified polynucleotides are collected and the purified
polynucleotides are analyzed for impurities. In the following Example, purified polynucleotides in the preparations of Example 1 or Example 2 and pressure filtered as described in Example 4, may be analyzed as in the following Example.
[0090] Coomassie-stained protein gels may be performed to determine the presence of residual proteins present before and after purifications. In some instances, BCA assays may be performed as well.
[0091] mRNA size and integrity7 may be assessed via gel electrophoresis. Either 1.0% agarose gel or Invitrogen E-Gel precast 1.2% agarose gels may be employed. mRNA is loaded at 1.0- 1.5 pg quantities per well. Upon completion, messenger RNA bands are visualized using ethidium bromide.
[0092] In vitro transfections of control iuciferase mRN A may be performed using HEK293T ceils. Transfections of l gg of each mRNA construct are performed in separate wells using a lipid based-transfection reagent according to manufacturer’s protocol. Cells are harvested at selected time points (e.g., 4 hour, 8 hour, etc.) and respective protein production is analyzed. For FFL mRNA, cell lysates are analyzed for Iuciferase production via bio luminescence assays. [00931 ΪΏ Examples measuring a control fluorescent RNA, a bioluminescence assay may be conducted using a Promega Luciferase Assay System (Item # El 500). The Luciferase Assay Reagent is prepared by adding Luciferase Assay Buffer to Luciferase Assay Substrate and mixing via a vortex.
[00941 Purified polynucleotides from Example 4 are loaded onto a 96-well plate followed by- plate control to each sample. Separately, Luciferase Assay Reagent (prepared as described above) is added to each well of a 96-well flat bottomed plate. Each plate is then inserted into the appropriate chambers using a Molecular Device Flex Station Instalment and the luminescence (measured in relative light units (RLUj) is measured.
EQUIVALENTS
[00951 .Although preferred embodiments of the invention have been described using specific terms, such description is for illustrative purposes only, and it is to be understood that changes and variations may be made without departing from the spirit or scope of the following claims.
INCORPORATION BY REFERENCE
[0096] The entire contents of all patents, published patent applications, and other references cited herein are hereby expressly incorporated herein in their entireties by reference.

Claims

1. A method of separating long polynucleotides from a composition, the method comprising:
introducing a composition including one or more long polynucleotides into a container including at least one boundary defined by a filter comprising a plurality of pores, wherein the pores have a smaller cross-sectional dimension than specified for the long polynucleotide’s molecular weight; and
applying elevated hydraulic pressure to the composition;
thereby causing at least some of the one or more long polynucleotides to pass through the pores.
2. A method of separating a long polynucleotide from a composition, the method comprising:
(a) providing a composition comprising a long polynucleotide;
(b) disposing the composition within a container including at least one boundary comprising a plurality of pores having a smaller cross-sectional dimension than specified for a molecular weight of the long polynucleotide; and
(c) subjecting the composition to elevated hydraulic pressure within the container under conditions to cause the long polynucleotide to pass through the pores;
thereby separating the long polynucleotide from the composition.
3. The method of claims 1 or 2, wherein the long polynucleotides have a length of about 1 kilobase or greater.
4. The method of claims 1 or 2, wherein the long polynucleotides have a length selected from the group consisting of: >950 kilobase, >900 kilobase, >850 kilobase, >800 kilobase, >750 kilobase, >700 kilobase, >650 kilobase, and >600 kilobase.
5. The method of claims 1 or 2, wherein the composition further comprises a second component.
6 The method of claim 4, wherein the second component does not pass through the pores.
7. The method of claims 1 or 2, wherein:
the filter is positioned within the container between an inlet and an outlet; and the composition is flowed over the filter.
8. The method of claim 7, wherein the composition is flowed laterally over the filter.
9. The method of claims 1 or 2, wherein the elevated hydraulic pressure is between about 0.1 and about 30 pounds per square inch (psi), inclusive.
10. The method of claims 1 or 2, wherein the elevated hydraulic pressure is below a pressure that would impact the stability of other components of the composition
11. The method of claims 1 or 2, wherein the long polynucleotides are sheared during passage through the pores.
12. The method of claims 1 or 2, wherein the pores have an effective molecular weight cutoff of about 1,000 kDa.
13. The method of claims 1 or 2, wherein the pores have a maximum cross-sectional dimension between about 50 nm and about 150 nm.
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