This application includes a Sequence Listing submitted electronically as a text file named 18804500101SEQ, created on Nov. 15, 2017 with a size of 45 kilobytes. The Sequence Listing is incorporated by reference herein.
The present disclosure relates generally to the field of vaccine manufacture. More particularly, the present disclosure relates to nanodisc carriers for vaccine antigens, which comprise a bilayer of thermostable phospholipids comprising ether linkages between the phosphate and hydrophobic side chains, scaffold proteins, and viral envelope protein antigens in their native conformation embedded within the carrier.
Various publications, including patents, published applications, accession numbers, technical articles and scholarly articles are cited throughout the specification. Each of these cited publications is incorporated by reference, in its entirety and for all purposes, in this document.
Classical methods of vaccine production use either modified live (e.g., attenuated) virus or killed (e.g., inactivated) virus to stimulate immunity. The development and accelerated production of safer and more stable vaccines is desirable for combatting highly virulent pathogens of interest. In addition, vaccines that are thermo-stable are needed for use and distribution in areas of the world where refrigeration is scarce and supplies must be stored in unregulated conditions where temperatures are well in excess of that required to maintain the potency of typical vaccine formulations. An example of the urgent need for such thermo-stable vaccines has been the Ebola outbreak in towns and remote villages of Africa.
Ebola virus (EBOV), a member of the order of enveloped viruses Mononegavirales, causes a severe hemorrhagic disease in humans, exhibiting mortality rates as high as 90%.1 This high mortality rate, combined with an absence of efficacious treatments or established vaccination options, makes Ebola virus a critical public health pathogen, and a bio threat pathogen of category A.
The EBOV surface glycoprotein (GP) mediates attachment to and fusion of the virus with host cells. GP is a type 1 transmembrane protein that is displayed on the virion envelope as a homo-trimeric spike, similar in fashion to several other envelope antigens (e.g., HIV Env and influenza virus hemagglutinin (HA)). The GP protein is exposed on the surface of Ebola virions, and it is widely recognized as the primary antigen of Ebola—thus vaccination with a purified, native-like but noninfectious protein is an obvious choice for an effective vaccination strategy.
The extracellular domain of the Zaire Ebola virus (ZEBOV) GP protein, lacking its transmembrane domain, has been fused to the Fc fragment of human IgG1 and the resultant fusion protein was successfully expressed in mammalian cells. Although this sort of soluble construct conferred protection to mice against a lethal viral challenge, it failed when similarly tested in non-human primates (NHP). Vaccines that utilize soluble forms of virion envelope antigens may not properly mimic the native structure of the membrane-integrated glycoprotein displayed on the virion for the purpose of immunization. This perspective is supported by studies in which antigens expressed in their native conformation are more effective at eliciting an effective immune response than in their non-native form. Indeed, virus-like particles (VLP) that present full-length, native GP on their surfaces have recently been demonstrated to be efficacious in eliciting protective immunity in NHP.
Although VLPs can be produced by transfecting mammalian cell lines with the EBOV matrix protein (VP40) and GP, VLPs are less than ideal vaccines for a number of reasons. Primarily, they are particulate in nature, and thus impossible to separate from other particulate contaminants like adventitious viruses. Because they have enclosed spaces it is exceedingly difficult to ensure the complete removal or inactivation of endogenous host nucleic acids or entrapped host proteins. Since the envelopes of VLPs are derived from the membrane of the host cell that produces them, they consequently contain many additional membrane-anchored or membrane-integrated proteins originating from the host cell membrane. Yet the success of using Ebola VLPs to elicit effective immune responses in NHP suggests that if envelope antigens could be highly purified and delivered in a vaccine in their native, membrane-embedded form, just as they are in VLPs, they may be equally effective in promoting protective immunity.
If envelope antigens could be delivered in a vehicle with built-in adjuvant properties, they might even prove more effective, and without the drawbacks of VLPs with respect to contamination with host-derived or potentially infectious, adventitious contaminants.
A thermostable vaccine carrier comprises a bilayer comprising one or more ether glycerophospholipids and one or more membrane scaffold proteins self-assembled into a nanodisc, and a microbial protein antigen embedded into the nanodisc. The one or more ether glycerophospholipids may comprise 1,2-di-O-phytanyl-sn-glycero-3-phosphocholine, 1,2-di-O-phytanyl-sn-glycerol, 1,2-di-O-phytanyl-sn-glycerol, 1,2-di-O-phytanyl-sn-glycero-3-phosphoethanolamine, glycerol dialkyl glycerol tetraether, 1,2-di-O-octadecyl-sn-glycero-3-phosphocholine, 1,2-di-O-(9Z-octadecenyl)-sn-glycero-3-phosphocholine, 2-3-diphytanyl-O-sn-glycerol (archaeol), caldarcheol, isocalarcheol, gentiobiosyl archaeol, archaetidylethanoloamine, or gentyobiosyl caldarc haetidylethanoloamine, or any combinations thereof. The membrane scaffold protein may comprise a polypeptide fragment of human apolipoprotein A1, or a variant thereof having one amino acid substitution or deletion. The membrane scaffold protein may comprise one or more of the amino acid sequence of SEQ ID NO:2, SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID NO:12, or SEQ ID NO:13.
The microbial protein antigen may comprise a virus envelope protein. The virus envelope protein may be from a DNA virus or an RNA virus. The virus envelope protein may be purified from a virus-like particle (VLP) as described herein. The DNA virus may be a herpesvirus, a poxsvirus, or a hepadnavirus. The RNA virus may be a togavirus, a coronavirus, an orthomyxovirus such as Influenza Type A, Influenza Type B, or Influenza Type C, a paramyxovirus, a rhabdovirus, a bunyavirus, a filovirus such as the Ebola virus, or a flavivirus such as the Zika virus. Preferred envelope proteins include the Influenza hemagglutinin protein (e.g., the amino acid sequence of SEQ ID NO:18), the Ebola VP40 protein (e.g., the amino acid sequence of SEQ ID NO:15), the Ebola GP protein (e.g., the amino acid sequence of SEQ ID NO:16), and the Zika virus envelope protein (e.g., the amino acid sequence of SEQ ID NO:17).
A composition comprises a thermostable vaccine carrier such as those described above, and a pharmaceutically acceptable carrier. The composition may further comprise a pharmaceutically acceptable excipient and/or an adjuvant.
A kit comprises a thermostable vaccine carrier or composition thereof such as those described above, and instructions for using the carrier in a method for vaccinating a subject in need thereof. The kit may comprise a container such as a syringe or diluent bag, and optionally comprise a needle or catheter for administering the thermostable vaccine carrier or composition to a subject.
A method for vaccinating a subject comprises administering to the subject a thermostable vaccine carrier or composition thereof such as those described above, in an amount effective to confer an immune response in/by the subject against the microbial protein antigen. Administration may be by injection. The injection may be a subcutaneous, intramuscular, or intravenous injection.
A thermostable vaccine carrier or composition thereof such as those described above may be used in the manufacture of a medicament or a vaccine. A thermostable vaccine carrier or composition thereof such as those described above may be used in the treatment or prevention of a virus infection or in the manufacture of a medicament or a vaccine for the treatment or prevention of a virus infection. A thermostable vaccine carrier or composition thereof such as those described above may be used in the treatment or prevention of a herpesvirus infection, a poxsvirus infection, a hepadnavirus infection, a togavirus infection, a coronavirus infection, an orthomyxovirus infection, a paramyxovirus infection, a rhabdovirus infection, a bunyavirus infection, a filovirus infection, or a flavivirus infection. A thermostable vaccine carrier or composition thereof such as those described above may be used in the treatment or prevention of an Ebola virus infection. A thermostable vaccine carrier or composition thereof such as those described above may be used in the treatment or prevention of a Zika virus infection. A thermostable vaccine carrier or composition thereof such as those described above may be used in the treatment or prevention of an Influenza virus infection.
A method for making a thermostable vaccine carrier such as those described above comprise mixing one or more ether glycerophospholipids, one or more membrane scaffold proteins, and one or more microbial protein antigens in an aqueous media comprising a detergent, removing the detergent, and allowing the one or more membrane scaffold proteins and the one or more ether glycerophospholipids to self-assemble into the nanodisc having the one or more microbial protein antigen embedded therein. The method may further comprise lyophilizing the nanodisc.
A process for producing substantially pure Ebola GP protein comprises transfecting Ebola VP40 protein-expressing stable cells with a gene encoding the Ebola GP protein, isolating virus-like particles comprising the Ebola VP40 protein and Ebola GP protein produced from the transfected cells, separating the GP protein from the VP40 protein, and purifying the separated GP protein. The stable cells may be Chinese Hamster Ovary (CHO) cells or Human Embryonic Kidney 293 (HEK 293) cells.
Various terms relating to aspects of the present disclosure are used throughout the specification and claims. Such terms are to be given their ordinary meaning in the art, unless otherwise indicated. Other specifically defined terms are to be construed in a manner consistent with the definition provided in this document.
As used throughout, the singular forms “a,” “an,” and “the” include plural referents unless expressly stated otherwise.
The terms subject and patient are used interchangeably. A subject may be any animal, and preferably is a mammal. A mammalian subject may be a farm animal (e.g., sheep, horse, cow, pig), a companion animal (e.g., cat, dog), a rodent or laboratory animal (e.g., mouse, rat, rabbit), or a non-human primate (e.g., old world monkey, new world monkey). Human beings are highly preferred.
A “phospholipid” includes a phosphate group joined to one or more, including two, hydrocarbon tails, which are typically long fatty acid chains that may be saturated or unsaturated. The phosphate group may further be joined to any suitable substituent group such as a choline, ethanolamine, glycerol, inositol, or serine. “Glycerophospholipids” are phospholipids including a glycerol group between the phosphate and two hydrocarbon tails (e.g., long fatty acid chains that may be saturated or unsaturated). “Ether phospholipids” include “ether glycerophospholipids,” in which one or more of the carbons on the glycerol group are joined to a hydrocarbon tail via an ether linkage.
A “nanodisc” comprises a bilayer of phospholipids, preferably glycerophospholipids and more preferably ether glycerophospholipids and one or more membrane scaffold proteins or peptides that form a belt-like perimeter around the hydrophobic edges of the bilayer (e.g.,
It was observed in accordance with the present disclosure that ether glycerophospholipids, together with membrane scaffold proteins, can be used to form nanodisc vaccine carriers. The nanodisc vaccine carriers self-assemble under aqueous conditions, and can be loaded with vaccine antigens, and administered to a subject as part of a vaccine in order to elicit a protective immune response. It was further observed that the use ether glycerophospholipids increases the thermostability of the nanodisc carrier relative to ester glycerophospholipids. It is believed that the presence of the ether linkage instead of the ester linkage significantly enhances the stability and shelf-life of the nanodisc structure, and further enhances the potency and efficacy of the vaccine that is administered, particularly in view of the immunogenic and potent adjuvant properties associated with archaebacterial/thermophilic bacterial lipids.
The nanodiscs prepared according to the present disclosure enable manufacturing of thermostable vaccines by incorporating viral envelope proteins in their native, substantially non-denatured conformation into the nanodiscs, providing for both thermostability and high immunogenicity. The present disclosure provides a highly extensible means to rapidly (within a few months) manufacture thermostable, potent vaccines to defend against infectious enveloped viruses, and uniquely provides the potential to be quickly reconfigured to incorporate new or altered antigens on very short notice. The present disclosure further enables the creation of highly multivalent configurations to adapt to rapidly changing antigen epitopes or multiple emergent bio threats.
The present disclosure presents several highly advantageous features to facilitate immunization against infectious agents, particularly enveloped viruses. Such advantageous features include, but are not limited to: The capacity to manufacture a vaccine using high cell mass electroporation to rapidly introduce the target envelope protein into VLPs, which can be purified and then used to extract the glycoprotein, then reconstitute it into nanodiscs of relatively standardized composition; The potency anticipated for nanodiscs incorporating archaebacterial lipids with adjuvant properties enables the incorporation of multiple DNA sequences in the transient transfection, permitting the manufacture of multivalent vaccines; The use of thermostable lipids confers thermostability to the nanodiscs, enabling the storage, shipment, and deployment of nanodisc-based vaccines in the field without the necessity for cryogenic or refrigerated storage; and the capacity to modify to develop and manufacture vaccines capable of inducing protective immunity to a wide variety of dangerously infectious enveloped vaccines.
Thus, in some embodiments, the present disclosure provides ether glycerophospholipid nanodiscs. The ether glycerophospholipid nanodiscs may be used, for example, as a carrier for vaccine antigens, and may provide the additional benefit of functioning as an adjuvant in a vaccine preparation. The ether glycerophospholipid nanodiscs are thermostable, particularly at elevated temperatures (e.g., those above room temperature, including temperatures at or above the temperature of the human body, 37 degrees C.). The ether glycerophospholipid nanodiscs are more thermostable than ester glycerophospholipid nanodiscs. Thus, the ether glycerophospholipid nanodiscs provide an improvement over the nanoscale particles described in U.S. Pat. No. 7,691,414, U.S. Pat. No. 7,662,410, U.S. Pat. No. 7,622,437, U.S. Pat. No. 7,592,008, U.S. Pat. No. 7,547,5763, U.S. Pat. No. 7,083,958, and U.S. Pat. No. 7,048,949.
In some embodiments, a thermostable vaccine carrier comprises a bilayer comprising one or more ether glycerophospholipids and one or more membrane scaffold proteins self-assembled into a nanodisc, and a microbial protein antigen embedded into the nanodisc. The ether glycerophospholipids may comprise any suitable ether glycerophospholipids that are found in the cell membrane of archaebacteria, particularly thermophilic archaebacteria. The ether glycerophospholipids may be synthetic. In some embodiments, ether glycerophospholipids that are found in the cell membrane of archaebacteria and synthetic ether glycerophospholipids may be used in combination. Non-limiting examples of suitable ether glycerophospholipids include 1,2-di-O-phytanyl-sn-glycero-3-phosphocholine, 1,2-di-O-phytanyl-sn-glycero-3-phosphoethanolamine, 1,2-di-O-phytanyl-sn-glycerol, glycerol dialkyl glycerol tetraether, 1,2-di-O-octadecyl-sn-glycero-3-phosphocholine, 1,2-di-O-(9Z-octadecenyl)-sn-glycero-3-phosphocholine, 2-3-diphytanyl-O-sn-glycerol (archaeol), caldarcheol, isocalarcheol, gentiobiosyl archaeol, archaetidylethanoloamine, gentyobiosyl caldarc haetidylethanoloamine, and any combination thereof.
The nanodisc may comprise any suitable shape, including a substantially round shape, an ovular or elliptical shape, a polygonal shape, or irregular shape. The nanodisc bilayer may comprise any suitable dimensions. The nanodisc bilayer may have a height of from about 1 nm to about 15 nm, preferably from about 1 nm to about 6 nm, from about 1 nm to about 5 nm, from about 2 nm to about 8 nm, from about 2 nm to about 6 nm, from about 3 nm to about 7 nm, from about 4 nm to about 6 nm, from about 4 nm to about 8 nm, from about 5 nm to about 10 nm, from about 5 nm to about 8 nm, from about 5 nm to about 7 nm, from about 6 nm to about 8 nm, from about 7 nm to about 10 nm, or from about 8 nm to about 10 nm though the nanodisc bilayer may have a height dimension greater than about 10 nm. The nanodisc bilayer may have a diameter, length, or width of from about 1 nm to about 20 nm, preferably from about 5 nm to about 15 nm, from about 5 nm to about 10 nm, from about 6 nm to about 12 nm, from about 6 nm to about 10 nm, from about 7 nm to about 15 nm, from about 7 nm to about 14 nm, from about 7 nm to about 13 nm, from about 7 nm to about 12 nm, from about 7 nm to about 11 nm, from about 7 nm to about 10 nm, from about 8 nm to about 15 nm, from about 8 nm to about 14 nm, from about 8 nm to about 13 nm, from about 8 nm to about 12 nm, from about 8 nm to about 11 nm, from about 8 nm to about 10 nm, about 9 nm to about 15 nm, from about 9 nm to about 14 nm, from about 9 nm to about 13 nm, from about 9 nm to about 12 nm, from about 9 nm to about 11 nm, or from about 10 nm to about 15 nm.
The structural integrity of the nanodisc, as well as the compatibility of the nanodisc with an aqueous environment (the edges of the nanodisc will comprise a hydrophobic character, particularly near the center, owing to the hydrophobic hydrocarbon tails) is mediated, in part, by the inclusion of membrane scaffold proteins (MSPs), which wrap around the perimeter of the nanodisc, akin to a belt (
The MSP may comprise human apolipoprotein A1, or may comprise a fragment (e.g., peptide fragment) of human apolipoprotein A1. Human apolipoprotein A1 may comprise the amino acid sequence of SEQ ID NO:14. The MSP may comprise a variant (e.g., comprise one or more amino acid substitutions, deletions, or insertions) of human apolipoprotein A1 or fragment (e.g., peptide fragment) thereof. The MSP may comprise SEQ ID NO:1, SEQ ID NO:2, SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID NO:12, or SEQ ID NO:13, or may comprise a fusion of one or more of SEQ ID NO:1, SEQ ID NO:2, SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID NO:12, or SEQ ID NO:13. Such a fusion may be direct (e.g., N-terminal to C-terminal linkage) or indirect (e.g., via a synthetic linker such as a Gly-Ser linker peptide).
The nanodisc preferably comprises a vaccine antigen. The vaccine antigen may comprise a protein or a polypeptide, including a glycoprotein, lipoprotein, and other proteins that may elicit an immune response.
In some embodiments, the vaccine antigen comprises a microbial protein, preferably a viral protein, more preferably a microbial protein, and more preferably a viral envelope protein. In some embodiments, the vaccine antigen comprises an envelope protein from a DNA virus. In some embodiments, the vaccine antigen comprises an envelope from an RNA virus.
DNA viruses having envelope proteins suitable for use in the nanodisc carrier include the herpesvirus, poxvirus, and hepadnavirus. RNA viruses having envelope proteins suitable for use in the nanodisc carrier include togavirus, coronavirus, orthomyxovirus, paramyxovirus, rhabdovirus, bunyavirus, filovirus, and flavivirus. In some embodiments, the orthomyxovirus is an Influenza virus, including an influenza type A virus, influenza type B virus, and influenza type C virus. In some embodiments, the filovirus is the Ebola virus. In some embodiments, the flavivirus is the Zika virus.
In some embodiments, the virus envelope protein comprises the Influenza virus hemagglutinin protein. The hemagglutinin protein may comprise the amino acid sequence of SEQ ID NO:18. In some embodiments, the virus envelope protein comprises the Ebola virus protein VP40 or the Ebola virus GP protein, or both the VP40 and GP protein may be included in the nanodisc carrier. The VP40 protein may comprise the amino acid sequence of SEQ ID NO:15. The GP protein may comprise the amino acid sequence of SEQ ID NO:16. In some embodiments, the virus envelope protein comprises the Zika virus envelope protein. The Zika virus envelope protein may comprise the amino acid sequence of SEQ ID NO:17. Such viral envelope proteins may be recombinantly expressed, for example, via a virus-like nanoparticle (VLP) or via a nano-VLP, with the envelope protein purified, isolated, or otherwise obtained from the VLP or nano-VLP.
The viral envelope protein is preferably embedded in the nanodisc. The viral envelope protein is preferably embedded in the ether glycerophospholipid bilayer, for example, on either or both the top or bottom leaflet of the bilayer. For example, a hydrophobic portion of the envelope protein may be embedded within the hydrophobic center area of the bilayer (among the hydrophobic tails). It is preferred that the envelope protein is embedded in the bilayer in substantially the envelope protein's native conformation and that the protein is not substantially denatured. The protein also substantially retains its native conformation once embedded in the bilayer, as well as during storage of the nanodisc. Thus, the loading process does not substantially denature the viral envelope protein (e.g., exposure to detergents and/or high temperatures and/or detergent removing reagents during nanodisc preparation and self-assembly does not substantially denature the viral envelope protein (or the MSP)).
More than one viral envelope protein may be embedded in the nanodisc carrier. Thus, the vaccine may comprise multiple viral envelope proteins, and may comprise multiple different viral envelope proteins (e.g., for an Ebola virus vaccine, both the GP protein and the VP40 protein may be embedded in the nanodisc carrier).
The nanodiscs, including the viral envelope protein embedded therein, may be included in a composition comprising the nanodisc and a carrier, as well as one or more excipients, an adjuvant, or one or more excipients and an adjuvant (as the nanodiscs may have adjuvant qualities, the composition may comprise a separate adjuvant). The carrier is preferably a pharmaceutically acceptable carrier, preferably an aqueous carrier, and is preferably suitable for parenteral administration. Suitable carriers include any media that does not interfere with the antigenic character of the viral envelope protein and does not interfere with the capacity of the nanodisc+envelope protein to elicit a protective immune response, and preferably is not toxic to the subject to which it is administered. The carrier may comprise water, saline, or an aqueous alcohol, or a physiologically compatible buffer, such as Hanks's solution, Ringer's solution, or physiological saline buffer. The carrier may contain formulatory agents, such as suspending, stabilizing and/or dispersing agents. The carrier may also include a buffer or a pH adjusting agent. The buffer may be a salt prepared from an organic acid or base. Representative buffers include organic acid salts, such as salts of citric acid, ascorbic acid, gluconic acid, carbonic acid, tartaric acid, succinic acid, acetic acid, or phthalic acid, Tris, tromethamine hydrochloride, or a phosphate buffer. Preparations for parenteral administration include sterile solutions ready for injection, and sterile dry nanodiscs ready to be combined with a carrier just prior to use.
Nanodiscs as described and as exemplified herein, including the viral envelope protein embedded therein, may be used as vaccines, and administered to a subject in an amount effective to elicit a protective immune response against the viral envelope protein antigen that further protects the subject from infection by the virus from which the viral envelope protein is a part. The nanodiscs may be administered to the subject as a composition comprising a carrier, excipient, and/or adjuvant. Thus, the present disclosure provides methods for vaccinating a subject in need thereof.
In some embodiments, methods for vaccinating a subject in need thereof comprise administering to the subject an effective amount of any nanodisc comprising any microbial protein or viral envelope protein described or exemplified herein. The effective amount may comprise any amount sufficient to elicit a protective immune response that protects the subject from infection by the virus from which the microbial protein or viral envelope protein is a part. The nanodisc may be comprised in a composition comprising a carrier, excipient, and/or adjuvant. The nanodisc, or composition thereof, is preferably administered parenterally, which may comprise a subdermal, subcutaneous, intramuscular, intravenous, or intra-arterial injection. The administering step may be repeated any number of times (e.g., repeat once, twice, three, four, or more times) sufficient to confer or maintain protective immunity (e.g., boostering). Repeat administration may follow any suitable period of time, for example, a month, two months, three months, six months, twelve months, eighteen months, twenty four months, or longer periods (e.g., several years).
The present disclosure also provides kits. The kits comprise any nanodisc comprising any microbial protein or viral envelope protein described or exemplified herein, or composition thereof, and instructions for using the nanodisc or composition thereof in a method for vaccinating a subject in need thereof. The kits may further comprise a carrier or diluent for mixing together with the nanodiscs prior to administration. The kits may further comprise a container housing the nanodisc or composition thereof, for example, a syringe, vial, or diluent bag, and may further comprise a needle or catheter for administering the nanodisc or composition thereof to a subject.
Any nanodisc comprising any microbial protein or viral envelope protein described or exemplified herein may be for use in the manufacture of a medicament or a vaccine in the treatment or prevention of a viral infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a herpesvirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a poxvirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a hepadnavirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a togavirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a coronavirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a orthomyxovirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a paramyxovirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a rhabdovirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a bunyavirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a filovirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a flavivirus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of an influenza type A virus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of an influenza type B virus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of an influenza type C virus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of an Ebola virus infection. The nanodiscs comprising a viral envelope protein may be for use in the treatment or prevention of a Zika virus infection.
The present disclosure also provides methods for preparing thermostable nanodisc vaccines. In general, the methods comprise mixing one or more membrane scaffold proteins (MSP), one or more microbial proteins e.g., one or more viral envelope proteins, and one or more ether glycerophospholipids together in an aqueous media comprising a detergent, removing the detergent and allowing the one or more membrane scaffold proteins and the one or more ether glycerophospholipids to self-assemble into a thermostable nanodisc comprising the one or more microbial proteins e.g., one or more viral envelope proteins, embedded therein, thereby forming a thermostable nanodisc vaccine. The one or more membrane scaffold proteins may comprise any membrane scaffold protein described or exemplified herein, the one or more ether glycerophospholipids may comprise any ether glycerophospholipid described or exemplified herein, and the microbial protein may comprise any microbial protein described or exemplified herein, including any viral envelope protein described or exemplified herein. Optionally, the thermostable nanodisc vaccine may be dried or lyophilized, then later reconstituted, for example, as a composition comprising a pharmaceutically acceptable carrier and/or excipient and/or adjuvant for administration as part of a vaccine regimen. In the nanodisc prepared according to the method, the microbial protein substantially retains its native conformation, as the protein is not substantially denatured during the mixing, detergent removal, or self-assembly steps.
During the step of mixing one or more membrane scaffold proteins (MSP), one or more microbial proteins e.g., one or more viral envelope proteins, and one or more ether glycerophospholipids together, the ratio of phospholipids to MSP may be from about 20:1 to about 200:1 (phospholipids:MSP), including from about 20:1 to about 180:1, from about 20:1 to about 150:1, from about 20:1 to about 100:1, from about 20:1 to about 80:1, from about 20:1 to about 50:1, from about 20:1 to about 40:1, from about 40:1 to about 200:1, from about 40:1 to about 160:1, from about 40:1 to about 140:1, from about 40:1 to about 120:1, from about 40:1 to about 100:1, from about 40:1 to about 80:1, from about 40:1 to about 60:1, from about 50:1 to about 200:1, from about 50:1 to about 150:1, from about 50:1 to about 100:1, from about 50:1 to about 75:1, from about 60:1 to about 200:1, from about 60:1 to about 180:1, from about 60:1 to about 120:1, from about 60:1 to about 90:1, from about 80:1 to about 200:1, from about 80:1 to about 190:1, from about 80:1 to about 180:1, from about 80:1 to about 160:1, from about 80:1 to about 120:1, from about 80:1 to about 100:1, from about 100:1 to about 200:1, from about 100:1 to about 150:1, from about 100:1 to about 125:1, from about 100:1 to about 120:1, from about 120:1 to about 200:1, from about 120:1 to about 180:1, from about 120:1 to about 160:1, from about 125:1 to about 150:1, from about 140:1 to about 180:1, from about 140:1 to about 160:1, from about 150:1 to about 200:1, or from about 180:1 to about 200:1. The ratio may vary, for example, based on the phospholipid used, the MSP used, or both the phospholipid and MSP used.
The ratio of microbial protein antigen (e.g., viral envelope protein) to MSP may be from about 1:2 to about 1:20 (antigen:MSP), from about 1:2 to about 1:18, from about 1:2 to about 1:16, from about 1:2 to about 1:14, from about 1:2 to about 1:12, from about 1:2 to about 1:10, from about 1:2 to about 1:8, from about 1:2 to about 1:6, from about 1:2 to about 1:4, from about 1:3 to about 1:18, from about 1:3 to about 1:15, from about 1:3 to about 1:12, from about 1:3 to about 1:9, from about 1:3 to about 1:6, from about 1:4 to about 1:16, from about 1:4 to about 1:12, from about 1:4 to about 1:8, from about 1:5 to about 1:20, from about 1:5 to about 1:15, from about 1:5 to about 1:10, from about 1:6 to about 1:17, from about 1:6 to about 1:11, from about 1:8 to about 1:18, from about 1:8 to about 1:16, from about 1:8 to about 1:12, from about 1:10 to about 1:20, from about 1:10 to about 1:15, from about 1:10 to about 1:12, from about 1:12 to about 1:16, from about 1:12 to about 1:14, from about 1:13 to about 1:16, from about 1:13 to about 1:15, from about 1:15 to about 1:20, from about 1:15 to about 1:18, from about 1:16 to about 1:20, or from about 1:16 to about 1:18.
Nanodisc assembly temperature may depend, for example, on the particular lipid. The temperature may range from about 4 degrees C. to about 50 degrees C., from about 25 degree C. to about 50 degrees C., from about 25 degree C. to about 37 degrees C., from about 25 degrees C. to about 40 degrees C., from about 37 degrees C. to about 50 degrees C., or from about 37 degrees C. to about 45 degrees C. Assembly may be carried out at about 25 degrees C., at about 37 degrees C., at about 40 degrees C., at about 45 degrees C., or at about 50 degrees C.
For removing the detergent, the ratio of detergent-removing beads (e.g., AMBERLITE® beads) to detergent can be from about 10:1 to 100:1, from about 20:1 to about 90:1, from about 20:1 to about 80:1, from about 20:1 to about 60:1, from about 30:1 to about 90:1, from about 30:1 to about 80:1, from about 30:1 to about 70:1, or from about 25:1 to about 85:1.
The expression and ensuing oligomerization of the Ebola matrix protein VP40 is the only viral element required to drive formation of filamentous, enveloped VLPs that are subsequently discharged from cells. The efficiency of production of VLPs driven by the sole expression of VP40, however, is poor. VLP formation and release are dramatically increased by the presence of the GP envelope protein. The membrane-bound form of GP is believed to enhance VP40 VLP release.
Since expression of the GP protein adversely affects cells by a phenomenon termed GP-mediated cytopathology, the STEP® (Batavia Biosciences BV) platform technology may be used to construct a stable cell line that expresses VP40 alone (
Once the stable cell line is identified, a MAXCYTE STX® (MaxCyte, Inc.) high cell mass electroporation instrument (flow electroporation) is used to transiently transfect the VP40 expressing cells (e.g., CHO cells or HEK 293 cells) with GP DNA, thereby inducing the cells to produce high quantities of Ebola VLPs containing the GP antigen. The resultant VLPs are separated away from cells and other debris, and then, full-length GP antigen is purified from the VLPs. Purified GP protein may then be loaded/incorporated into the thermostable nanodiscs (e.g., those comprising ether glycerophospholipids for enhanced thermostability). An overview is presented in schematic form in
In some embodiments, Ebola VLPs are removed from the CHO or HEK 293 cells by filtration, and concentrated, for example, with tangential flow filtration. The highly pleiotropic distribution of particle sizes may be reduced to smaller size by sonication or micro fluidization (e.g., producing nano-VLPs), filtered through a glass-fiber filter, and then further purified through a cation exchange membrane filter (Sartorius) and a CAPTO® Core 700 column (GE HealthCare) to remove nucleic acids and residual host cell contaminants. The particles may be subjected to additional sonication or micro fluidization to reduce their overall size to a minimum, and then filtered through a 0.45 micron filter to reduce bio burden.
The purified VLPs may be extracted with a detergents, using both SDS-PAGE and ELISA analysis (e.g., using conformationally-sensitive monoclonal antibodies 13C6 and 6D3) so as to establish the best differential solubilization possible (e.g., identify the detergent that yields the highest recovery of conformationally-recognizable GP protein in highest relative quantity compared to all other VLP components). GP solubilized with detergent is further purified away from any other contaminants, with a major emphasis on exploiting its very large mass (˜600 kD) to achieve the separation. Chromatography on size-exclusion mixed chromatography resins (CAPTO® Core 700 and equivalent type resins) and entirely size-dependent size exclusion chromatography (SEC) exploit this feature of the protein in order to purify it away from contaminants. GP is very highly glycosylated (carbohydrates compose nearly half its mass) and lectin affinity chromatography may also be useful to enhance its purity as well. Additionally, once GP is solubilized with detergent, nanofiltration may be performed employing membranes with pores sufficiently small to exclude any viruses and virus-like particles, whether endogenous ones budded from the cells or others adventitious in nature. It is desirable to achieve a high degree of purity, taking care to incorporate steps intended to reduce contamination with undesirable contaminants such as nucleic acids and host cell proteins.
Once purified, the GP protein can be mixed with a membrane scaffold protein (MSP) and thermostable lipids (e.g., ether glycerophospholipids), including those analogous to the lipids found in archaebacteria as well as those semi-synthetically produced. Self-assembly of nanodiscs is initiated by the removal of detergent, and nanodiscs containing embedded single copies of trimeric GP are isolated from nanodiscs lacking GP protein by straightforward SEC using a SUPERDEX® column (GE Healthcare Bio-Sciences A.B.). The GP-containing nanodiscs can be aliquoted into various quantities in vials and lyophilized for storage. The final lyophilized product may be subsequently evaluated for thermostability and immunogenicity.
The procedures described above for GP protein may also be used in the preparation of nanodisc-based vaccines against other virus envelope antigens (e.g., HIV Env and influenza virus hemagglutinin (HA)). Furthermore, if the thermostable ether glycerophospholipids retain an adjuvant character similar to the adjuvant character observed for archaebacterial lipids, the potency of the resultant vaccines may enable transfection with not only a single DNA sequence, but many sequences coding for variants of the corresponding envelope antigen. For Ebola, this would mean transfecting not only with the sequence of the GP protein found in Zaire, but also with the sequences of GP present in the other four known strains, and/or with any new emergent infectious strain or variant. A similar strategy is followed for other enveloped viruses possessing antigens with extensive variability or drift in the viral strains encountered in the field.
The present disclosure also provides processes for producing Ebola GP protein, comprising transfecting an Ebola VP40 protein-producing stable CHO cell with a gene encoding the Ebola GP protein, isolating VLPs comprising Ebola VP40 protein and Ebola GP protein produced from the transfected CHO cell, separating the GP protein from the VP40 protein, and purifying the separated GP protein.
VLPs are used as a highly enriched source from which viral envelope protein antigens can be purified following their extraction and solubilization with detergent. Once purified to biopharmaceutical standards, the envelope protein can be loaded into a thermostable nanodisc carrier in a way that resembles or mimics the natural environment or habitat that the envelope protein experiences in the virion.
The present disclosure also provides CHO or HEK 293 cells stably transformed with a gene encoding the Ebola virus VP40 protein, or with a gene encoding the Ebola virus GP protein, or with a gene encoding the Ebola virus VP40 protein and the Ebola virus GP protein, which cells express the VP40 protein, or express the GP protein, or express both the VP40 protein and the GP protein. Such cells, and methods for producing them, are provided.
The following representative embodiments are presented:
A thermostable vaccine carrier, comprising a bilayer comprising one or more ether glycerophospholipids and one or more membrane scaffold proteins self-assembled into a nanodisc, and a microbial protein antigen embedded into the nanodisc.
The thermostable vaccine carrier according to embodiment 1, wherein the one or more ether glycerophospholipids is selected from the group consisting of 1,2-di-O-phytanyl-sn-glycero-3-phosphocholine, 1,2-di-O-phytanyl-sn-glycero-3-phosphoethanolamine, glycerol dialkyl glycerol tetraether, 1,2-di-O-octadecyl-sn-glycero-3-phosphocholine, 1,2-di-O-(9Z-octadecenyl)-sn-glycero-3-phosphocholine, 2-3-diphytanyl-O-sn-glycerol (archaeol), caldarcheol, isocalarcheol, gentiobiosyl archaeol, archaetidylethanoloamine, gentyobiosyl caldarc haetidylethanoloamine, and combinations thereof.
The thermostable vaccine carrier according to embodiment 1 or 2, wherein the one or more ether glycerophospholipids comprises 1,2-di-O-phytanyl-sn-glycero-3-phosphocholine.
The thermostable vaccine carrier according to embodiment 1 or 2, wherein the one or more ether glycerophospholipids comprises 1,2-di-O-phytanyl-sn-glycero-3-phosphoethanolamine.
The thermostable vaccine carrier according to embodiment 1 or 2, wherein the one or more ether glycerophospholipids comprises glycerol dialkyl glycerol tetraether.
The thermostable vaccine carrier according to any one of embodiments 1 to 5, wherein the membrane scaffold protein comprises a human apolipoprotein A1 fragment peptide or a variant thereof having one amino acid substitution or deletion.
The thermostable vaccine carrier according to any one of embodiments 1 to 6, wherein the membrane scaffold protein has the amino acid sequence of SEQ ID NO:1.
The thermostable vaccine carrier according to any one of embodiments 1 to 6, wherein the human apolipoprotein A1 fragment peptide has an amino acid sequence selected from the group consisting of SEQ ID NO:2, SEQ ID NO:3, SEQ ID NO:4, SEQ ID NO:5, SEQ ID NO:6, SEQ ID NO:7, SEQ ID NO:8, SEQ ID NO:9, SEQ ID NO:10, SEQ ID NO:11, SEQ ID NO:12, and SEQ ID NO:13.
The thermostable vaccine carrier according to any one of embodiments 1 to 8, wherein the microbial protein antigen is a virus envelope protein.
The thermostable vaccine carrier according to any one of embodiments 1 to 8, wherein the microbial protein antigen is a virus envelope protein, and the virus is a DNA virus.
The thermostable vaccine carrier according to embodiment 10, wherein the DNA virus is a herpesvirus.
The thermostable vaccine carrier according to embodiment 10, wherein the DNA virus is a poxsvirus.
The thermostable vaccine carrier according to embodiment 10, wherein the DNA virus is a hepadnavirus.
The thermostable vaccine carrier according to any one of embodiments 1 to 8, wherein the microbial protein antigen is a virus envelope protein, and the virus is an RNA virus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a togavirus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a coronavirus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is an orthomyxovirus.
The thermostable vaccine carrier according to embodiment 17, wherein the orthomyxovirus is an Influenza virus.
The thermostable vaccine carrier according to embodiment 18, wherein the Influenza virus envelope protein is hemagglutinin and comprises the amino acid sequence of SEQ ID NO:18.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a paramyxovirus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a rhabdovirus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a bunyavirus.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a filovirus.
The thermostable vaccine carrier according to embodiment 23, wherein the filovirus is Ebola virus.
The thermostable vaccine carrier according to embodiment 24, wherein the Ebola virus envelope protein is VP40 and comprises the amino acid sequence of SEQ ID NO:15.
The thermostable vaccine carrier according to embodiment 24, wherein the Ebola virus envelope protein is GP and comprises the amino acid sequence of SEQ ID NO:16.
The thermostable vaccine carrier according to embodiment 14, wherein the RNA virus is a flavivirus.
The thermostable vaccine carrier according to embodiment 27, wherein the flavivirus is Zika virus.
The thermostable vaccine carrier according to embodiment 28, wherein the Zika virus envelope protein comprises the amino acid sequence of SEQ ID NO:17.
A composition, comprising the thermostable vaccine carrier according to any one of embodiments 1 to 29 and a pharmaceutically acceptable carrier.
The composition according to embodiment 30, further comprising a pharmaceutically acceptable excipient.
The composition according to embodiment 30 or 31, further comprising an adjuvant.
A kit, comprising the thermostable vaccine carrier according to any one of embodiments 1 to 26, a container containing the carrier, and instructions for using the carrier in a method for vaccinating a subject in need thereof.
The kit according to embodiment 33, wherein the thermostable vaccine carrier is comprised in a composition comprising a pharmaceutically acceptable carrier and optionally a pharmaceutically acceptable excipient, an adjuvant, or a pharmaceutically acceptable excipient and an adjuvant.
The kit according to embodiment 33 or 34, wherein the container comprises a syringe or diluent bag, and further comprising a needle or catheter for administering the thermostable vaccine carrier or composition to a subject in need thereof.
A method for vaccinating a subject in need thereof, comprising administering to the subject the thermostable vaccine carrier according to any one of embodiments 1 to 29 in an amount effective to confer an immune response against the microbial protein antigen in the subject.
The method according to embodiment 36, wherein the thermostable vaccine carrier is comprised in a composition comprising a pharmaceutically acceptable carrier and optionally a pharmaceutically acceptable excipient, an adjuvant, or a pharmaceutically acceptable excipient and an adjuvant.
The method according to embodiment 36 or 37, wherein the administering comprises injecting the thermostable vaccine carrier or composition subcutaneously, intramuscularly, or intravenously in the subject.
Use of the thermostable vaccine carrier according to any one of embodiments 1 to 29 in the manufacture of a medicament or a vaccine.
Use of the thermostable vaccine carrier according to any one of embodiments 1 to 29 in the treatment or prevention of a virus infection.
Use of the thermostable vaccine carrier according to embodiment 11 in the treatment or prevention of a herpesvirus infection.
Use of the thermostable vaccine carrier according to embodiments 12 in the treatment or prevention of a poxsvirus infection.
Use of the thermostable vaccine carrier according to embodiment 13 in the treatment or prevention of a hepadnavirus infection.
Use of the thermostable vaccine carrier according to embodiment 15 in the treatment or prevention of a togavirus infection.
Use of the thermostable vaccine carrier according to embodiment 16 in the treatment or prevention of a coronavirus infection.
Use of the thermostable vaccine carrier according to embodiment 17 in the treatment or prevention of an orthomyxovirus infection.
Use of the thermostable vaccine carrier according to embodiment 18 or embodiment 19 in the treatment or prevention of an Influenza virus infection.
Use of the thermostable vaccine carrier according to embodiment 20 in the treatment or prevention of a paramyxovirus infection.
Use of the thermostable vaccine carrier according to embodiment 21 in the treatment or prevention of a rhabdovirus infection.
Use of the thermostable vaccine carrier according to embodiment 22 in the treatment or prevention of a bunyavirus infection.
Use of the thermostable vaccine carrier according to embodiment 23 in the treatment or prevention of a filovirus infection.
Use of the thermostable vaccine carrier according to anyone of embodiments 24 to 26 in the treatment or prevention of an Ebola virus infection.
Use of the thermostable vaccine carrier according to embodiment 27 in the treatment or prevention of a flavivirus infection.
Use of the thermostable vaccine carrier according to embodiment 28 in the treatment or prevention of a Zika virus infection.
A method for making thermostable vaccine carrier according to any one of embodiments 1 to 29, comprising mixing the one or more ether glycerophospholipids, the one or more membrane scaffold proteins, and the microbial protein antigen in an aqueous media comprising a detergent, removing the detergent, and allowing the one or more membrane scaffold proteins and the one or more ether glycerophospholipids to self-assemble into the nanodisc having the microbial protein antigen embedded therein.
The method according to embodiment 55, further comprising lyophilizing the nanodisc.
A process for producing substantially pure Ebola GP protein, comprising transfecting Ebola VP40 protein-expressing stable cells with a gene encoding the Ebola GP protein, isolating virus-like particles comprising the Ebola VP40 protein and Ebola GP protein produced from the transfected cells, separating the GP protein from the VP40 protein, and purifying the separated GP protein.
The process according to embodiment 57, wherein the stable cells are Chinese Hamster Ovary (CHO) cells.
Mammalian cells stably transformed with a recombinant gene encoding the Ebola virus VP40 protein.
The mammalian cells according to embodiment 59, further transformed with a recombinant gene encoding the Ebola virus GP protein.
The mammalian cells according to embodiment 59 or 60, wherein the cells are Chinese Hamster Ovary (CHO) cells or Human Embryonic Kidney 293 (HEK 293) cells.
The following examples are provided to describe the subject matter in greater detail. They are intended to illustrate, not to limit, the claimed subject matter.
Since Ebola VLPs are a source from which the antigenic component of the vaccine (GP) is prepared, it is desirable to develop a robust approach to produce such VLPs in sufficient quantities. While there are many reports of Ebola VLPs being prepared by transient transfection of HEK293 cells, the approach has been described as complicated by inefficient and poorly reproducible transfection results and low yields. It is believed that this may be explained, at least in part, by the phenomenon termed GP-mediated cytopathology, as well as the difficulty of expanding cells post-transfusion due to the high burden placed upon them by the continual efflux of eVLPs budding from their cell membrane.
Recent improvements in flow electroporation methodology have enabled the transient transfection of very high-density cell cultures, ranging up to 1×1011 cells. The technology involves the application of an electric field to a cell suspension, causing the membranes of the cells to become transiently permeable, encouraging exogenous DNA to enter the cell. Optimization of the technique has led to the routine achievement of loading efficiencies exceeding 90%, and provided an avenue to successfully transform cells where reproducibility, efficiency, and the need for increased cell numbers are important.
Flow electroporation significantly improves both the reliability and yield of VLPs. One drawback of this technology is the large quantities of purified DNA that the electroporation requires when used to transiently transfect high-density cell cultures. A second drawback is that to produce VLPs decorated with GP, the host cells must be coerced to express the matrix protein, VP40 as well as the envelope antigen, GP. This doubles the amount of DNA required, and now that two species of DNA are required, it necessitates careful optimization and control of both the ratio and quantities of DNA. While such a co-transfection approach is pursued to obtain material to develop purification processes for the VLPs and GP protein, a stable cell line was constructed, which solely expresses the VP40 matrix protein, thus requiring only transfection with a single DNA sequence encoding the full-length GP protein to produce VLPs decorated with GP.
USAMRID has supplied two plasmids encoding for VP40 and GP, which is amplified to produce sufficient plasmid DNA to enable experiments to optimize parameters for large-scale production of Ebola VP. Three small-scale transient transfections using OC-400 cassettes for optimizing various parameters are performed, followed by six large-scale transfections using CL-2 bags.
A. Co-Transfection Methodology
In the first small-scale experiment, the optimal ratios and quantities of DNA needed to attain maximal VLP productivity are determined. A total of twelve transfections are performed per cell line (CHO cells and HEK 293 cells); nine comprise varying the total amount of DNA employed (ranging from 200 to 400 micrograms) and their ratios (evaluating 2:1, 1:1, and 1:2). The remaining three transfections are control-related to ensure the absence of any issues with the performance of the equipment.
A second optimization experiment explores the feasibility of first transfecting with VP40 DNA, and then conducting a second transfection with GP DNA after the cells are allowed to recover for periods of 5, 24, or 48 hours. In this experiment whether secondary transfection with DNA encoding the viral nucleoprotein (NP) further enhances VLP productivity is explored.
In the third small-scale transfection whether overall VLP productivity can be enhanced by inclusion of lipid supplements to the media post-transfection is evaluated. The intent is to promote the general well-being and longevity of cells that are constantly burdened with budding and discharging VLPs from their membranes.
After determining optimal parameters, six larger-scale co-transfections are performed to supply material to jump-start development and refinement of processes to isolate and purify VLPs and the GP protein.
B. Stable VP40 Cell Line Construction
To accelerate the construction and development of a stable cell line expressing VP40, STEP® technology (Batavia Bioservices BV Corp., Netherlands) a rapid plasmid-based system for generating high expressing, protein producing, mammalian (CHO) cell lines, is employed. The detailed preparation and materials used in the STEP® technology provided in U.S. Publ. No. 2012/156672, U.S. Publ. No. 2013/157312, and U.S. Publ. No. 2013/-23695.
An efficient selection system creating stably transfected mammalian cell lines requires killing un-transfected cells and achieving high protein expression levels.
The STEP® plasmid contains a very efficient, yet flexible, stringent cell selection system. Due to the translation of functionally impaired selection marker proteins, STEP® procedures eliminate un-transfected cells and low-expressing cells. Only cells that have very high mRNA expression levels are able to survive selective pressure—eliminating low-expressing cell lines, therefore greatly reducing the number of cell lines that need to be screened.
The Gene of Interest (GOI), encoding the desired therapeutic protein, is inserted into the plasmid using standard DNA approaches. The functionally impaired Zeocin (FI-Zeo) selection marker and DNA spacer create the highly stringent selection system. Linkage of the FI-Zeo marker to GOI via an internal ribosomal entry site (IRES) sequence results in high GOI expression, one RNA. The novel expression-enhancing (EE) elements, flanking the gene of interest (GOI), increase gene expression and allow cells to survive under high stringency (see
In the STEP® procedure, three different Zeocin selection protein mutants—noted as low, medium, and high stringency—are spliced into different cassettes to ensure success in any transfection. The lowest stringency plasmid produces the highest number of clones. The higher the stringency, fewer surviving clones are produced, but with potentially higher expression. However, when this strategy was successfully used to express difficult to produce proteins such as Factor VIII, high expressing clones were obtained only at the lowest stringency. There were no surviving clones at the medium or highest stringency. In the case of a less difficult protein, EPO, all three stringencies produced clones, but the highest levels of EPO were produced at the highest level of expression.
The VP40 gene is synthesized at a vendor of choice according to regulations intended to achieve TSE-risk reduction. The synthetic gene is cloned into three STEP® vectors with low, intermediate, and high stringencies, using materials without components of animal origin. Use of restriction endonucleases are performed and DNA gel electrophoresis according to in-house BBI protocols. After the final construction step is completed, the STEP® vectors are treated with chaotropic salts and transformed into animal-component-free competent E. coli. Colonies are picked and grown under TSE-free conditions, and DNA are extracted by midi prep and checked for both gene and element integrity by digestion analysis.
GMP CHO cells, in culture for 2-2.5 weeks after revival, are concentrated for the transfection to ˜1.3×106 vc/ml. A total of 1.5 ml of cells are centrifuged in 1.5 ml sterile tubes, thereby attaining ˜2×106 CHO cells per sample with 5 μg DNA. A total of 14 nucleofections are performed for pool generation following BBI protocols: 4× nucleofections: STEP®-VP40 (lowest stringency); 4× nucleofections: STEP®-VP40 (intermediate stringency); 4× nucleofections: STEP®-VP40 (highest stringency); 1× nucleofection of STEP® plasmid (lowest stringency) lacking GOI (Null Cell Line); and 1× nucleofection of cells only; the latter two are controls.
Following drug restriction, surviving pools are expanded and serially diluted into a total of twenty 96 well plates at 0.3 cells per well, or −30 cells per 96 well plate. A visual assessment of each well is conducted to ensure clonality. A total of 150 clones are expanded. If only the low stringency pools survive, than 150 clones from this level are continued. If all three stringencies produce pools, then 50 clones are continued from each level of stringency.
The 150 pools are expanded and transiently transfected in cuvettes with the GP-containing plasmid in groups of 24. On harvest day, the spent medium are centrifuged and or filtered to remove cells. Each clone is analyzed in triplicate by ELISA to determine the clones that produce the highest amount of GP-containing VLPs. The top 24 clones are expanded, cryopreserved and transiently transfected with GP DNA using MAXCYTE® cassettes (MaxCyte, Inc). Each clone is analyzed by ELISA to determine the highest titer in a larger scale transfection versus the cuvette. The highest expressing clone is expanded and transfected with GP DNA in CL-2 bags producing 4-5 liters of product. This is repeated a second time before executing the final transfection at twice the volume using GP DNA manufactured with very low endotoxin levels.
The selected clone is that stable clone which expresses VP40 matrix protein in such a fashion as to maximize VLP production upon introduction of GP DNA by flow electroporation transfection.
The construction of a stable VP40 cell line enables the production of VLPs decorated with whatever envelope protein is encoded by the DNA introduced in the transfection; modifying the DNA sequence to correspond to a new emergent strain or using a collection of very similar sequences to provide immunity against several closely related strains now becomes a straightforward option.
Using VLPs produced by large-scale (5 liters), nano-VLPs are produced as described below. A dead-end filtration process is configured to replace the initial low-speed centrifugation to remove cells and debris while tangential flow filtration is used instead of high-speed centrifugation to concentrate the VLPs. These changes render the process more scalable and suitable for manufacturing.
Once concentrated, the VLPs are sonicated to convert them into smaller species, termed Nano-VLPs. The process of sonication also considerably reduces their size distribution. The Nano-VLPs are then filtered through a glass-fiber, capsule filter, and subsequently subjected to flow-through chromatography using a cation-exchange membrane device (Sartobind S), and a novel CAPTO® Core 700 (GE Healthcare) column to remove nucleic acids and other smaller contaminants. The Nano-VLPs are sonicated a second time and then the bio burden is reduced by filtration through a 0.45 micron filter.
GP is a predominant component of the Nano-VLPs; only the highly oligomeric VP40 matrix protein is present in greater amounts (
Once Nano-VLPs are highly purified, differential solubilization of the protein from most of the other components of the VLPs can be achieved using a number of non-ionic detergents, (e.g., dodecyl-maltoside or octyl-glucoside are two representative candidates).
Since native GP protein is a very large homotrimer; once it is solubilized into a monodisperse form with detergent, its Stokes radius or apparent size are in excess of 600 kD. This property can be effectively leveraged to purify the protein away using two different strategies. The first involves performing simple molecular sieve or size exclusion chromatography (SEC), in which molecules are separated primarily according to their size. A second approach is to pass the solubilized extract through a new class of size-excluding adsorptive media (CAPTO® Core 700). The CAPTO® Core 700 chromatography column was designed for intermediate purification and polishing of viruses and large biomolecules. The media consists of a ligand-activated core that is enclosed by an inactive shell that excludes large molecules from entering the core through its pores (with a cutoff of approximately 700 kD). Smaller impurities bind to the internalized octylamine ligands, which are both hydrophobic and positively charged. The multimodal ligands in the core of the resin particle are able to bind, and thus remove a variety of types of impurities over a broad range of pH and salt concentrations.
These two separate procedures are not mutually incompatible; they can be combined sequentially to separate the GP molecule from smaller (or potentially larger for SEC) impurities possessing the capability to bind either hydrophobic or negatively charged species. Nucleic acids possess that latter property, and such combination is capable of a major reduction of that irksome impurity.
Once the GP is rendered in monodisperse form by solubilization with detergent, primarily in detergent micelles, the GP protein are small enough to pass unhindered through membranes designed to trap and capture comparatively much larger particles, such as viruses and virus-like particles.
The same detergent used to solubilize and extract the GP protein likewise exerts a disruptive effect on any adventitious enveloped viruses, aiding in their inactivation and/or destruction.
Some biological organisms, members of a class of organisms known as extremophiles, are able to grow at remarkably high temperatures. These thermophilic organisms are predominantly Archaeobacteria. Their ability to survive in these hostile environments is at least in part due to possessing membranes of unusual structure and stability. Their membranes, unlike those of found in eubacteria and eukaryotic cells, contain phospholipids with several unique features.
The stereochemistry of their glycerol component is opposite in comparison, and their side-chains are attached via ether instead of ester bonds. Additionally the side-chains contain branched structures that are composed by stringing together isoprene units. These features decrease the fluidity of the membrane enabling thermal stability, and also help make these lipid components more resistant to degradation processes such as oxidation.
Thermostable nanodiscs use natural or semi-synthetic archaeobacterial lipids and incorporates them into nanodiscs together scaffold proteins (e.g., MSP) and the vaccine antigens. Exemplary semi-synthetic archaeobacterial lipids identified in the literature as being particularly immunogenic are gentiotriosylarchaeol, mannotriosyl-archaeol, archaetidylserine, and 2,3-diphytanyl-sn-glycerol-1-phospho-3′-sn-glycerol-1′-methylphosphate in mol % ratio 22.5/22.5/30/25. However, a number of other ether phospholipids that are currently commercially available are also useful. This includes those listed in Table 1 below. 1,2-di-O-phytanyl-sn-glycero-3-phosphocholine is a preferred phospholipid, referred to herein as PC*. Others can be custom-synthesized (e.g., with different polar groups like serine) starting with the 1,2-di-O-phytanyl-sn-glycerol shown as the structure at the bottom Table 1.
Archaeobacteria that grow at extremely high temperatures are rich in diether and tetraether lipids. In thermoacidophiles or hyperthermophilic neutrophiles, the polar lipids contain diphytanylglycerol diether lipids (typically, ˜5-10%) and dibiphytanylglycerol-tetraether lipids (typically ˜90-95%, at optimum growth). The main phospholipid (the bipolar tetraether, GDGT, a caldarchaeol) of Thermoplasma acidophilum is commercially available from Matreya, LLC. The structure of this tetraether phospholipid is shown in Table 2.
An ester-based phospholipid, 2-Oleoyl-1-palmitoyl-sn-glycero-3-phosphocholine (POPC), was used in parallel experiments. POPC has the structure shown in Table 3.
In such extreme thermophiles, the membrane is primarily composed of a single layer of bipolar tetraether lipids that span the entire membrane, rather than being organized as a lipid bilayer. This type of membrane structure confers additional stability at extreme temperatures. We construct nanodiscs that are analogous to those prepared with diether lipids using tetraether lipids. Additionally, mixtures of diether and tetraether lipids may still be useful to confer improved stability and/or immunopotency.
Nanodiscs were assembled with synthetic ester and ether lipids at select lipid:MSP ratio and temperature conditions selected based on the physical properties of the lipids and preliminary experiments. The fully assembled disc was purified from the unassembled proteins and lipids by Size Exclusion Chromatography.
The Following Stock and Working Solutions were Prepared:
A. Stock solution of 200 mM Na-cholate (17.22 g of sodium cholate (SAFC; Catalog #S1702-100G; Lot # SLBP3019V)) in 200 ml dI water. 0.22 μm filtered
B. Stock solution of 5 M NaCl (146.1 g of sodium chloride (Fisher Chemical; Catalog # L-23125; Lot #144826A)) in 500 ml dI water. 0.22 μm filtered
C. Stock solution of 10×TBS (Sigma; Catalog # T5912-1L; Lot # SLBN9754V)
D. Working solution of 100 mM Na-cholate+100 mM NaCl: 50 ml of (100 mM Sodium cholate+100 mM NaCl) solution was prepared by mixing 25 ml of 200 mM sodium cholate, 1 ml of 5 M NaCl and 24 ml dI water.
E. Working solution of 1×TBS: 100 ml 1×TBS was prepared by diluting 10 ml of 10×TBS in 90 ml dI water.
F. Working solution of 1×TBS+100 mM Na-cholate: 10 ml of buffer containing 1×TBS+100 mM Na-cholate was prepared by diluting 1 ml of 10×TBS and 200 mM Na-cholate in 4 ml dI water.
G. Lipids were as follows: POPC (Sigma; Catalog #42773-100MG; Lot # BCBQ7862V); 16:0 Diether PC* (Avanti Polar Lipids; Catalog #999992); and GDGT (Major phospholipid from Thermoplasma acidophilum) Matreya LLC; Catalog #1303; Lot #23412
2000 nmoles of lipids were aliquoted from chloroform stocks into 10-130 mm borosilicate test tubes and dried under a stream of pure Nitrogen to deposit a thin film of lipids on the walls of the tubes. The tubes were placed in a vacuum desiccator for 6-8 hours.
The dried lipids were removed from the desiccator and 40 μl of 100 mM sodium-cholate+100 mM NaCl buffer was added to each tube to reconstitute the lipids. The tubes were vortexed until no residue was seen on the walls of the tubes and sonicated for 30 minutes with intermittent vortexing in an 80 degrees F. water bath.
Reconstituted lipids were then mixed with 1×TBS and scaffold protein MSP1D1 (BioNanoCon, Lot #150221B or Sigma Catalog # M6574) and incubated at RT for 30 minutes. Disc reconstitution mixtures were prepared according to the recipe (all volumes in μl) shown in Table 4.
Detergent removal was achieved by direct addition of hydrophobic beads (AMBERLITE® XAD-2 beads (Rohm and Haas Co.)) to the disc reconstitution mixtures. A ratio of 50:1 (w/w) AMBERLITE® beads:detergent was used for detergent removal. Appropriate amount of dry AMBERLITE® XAD-2 beads (Rohm and Haas Co.) was weighed out in 2-ml microcentrifuge tubes with screw top caps, as shown in Table 5. After 5 hours of incubation at 37 degrees C. on a shaker, the AMBERLITE® beads were removed using a filter. Spent beads were washed with 1×TBS on the filter itself to make the total volume of each solution 600 Samples were stored at 4° C. until further use.
The nanodiscs obtained from removing the AMBERLITE® beads (the filtrate) were purified using a SUPERDEX® 200 10/300 GL column (GE Healthcare Bio-Sciences A.B.) running 1×TBS at 0.75 ml/min. The purified nanodisc solution was stored at 4 degrees C. Purified nanodiscs were assessed using Size Exclusion Chromatography (SEC), as shown in
The size exclusion chromatogram profile of PC* nanodiscs was very similar to that obtained for POPC Nanodiscs with identical retention volumes. Four fractions around the main peak which were expected to contain the well assembled nanodiscs were pooled (Table 6) and used for thermostability assessment. Amount determination was made by using an extinction coefficient at 280 nm of 0.8515 mg/ml.
Purified POPC and PC* Nanodisc preparations were divided into 21 equal fractions, each in separate screw-top microcentrifuge tubes. Table 7 describes the pool fractions. Heat blocks were used for the study, and the nanodiscs were tested at room temperature, 37 degrees C., 50 degrees C., and 60 degrees C. Samples were taken at time zero (before heat exposure), and then after 30 minutes, 60 minutes, one hundred twenty minutes, twenty four hours, and forty eight hours of exposure to the heat conditions. All samples were analyzed at the same time at the end of the experiment. Samples were stored at 4° C. until that time.
Samples were transferred to a 96-well plate and analyzed via Analytical SEC on a SUPERDEX® 200 Increase 5/150 GL column (GE Healthcare Bio-Sciences A.B.) running 100 mM sodium phosphate, 150 mM sodium chloride solution pH 7.2 at 0.45 ml/min Integrity of the main peak was used as a measure of thermostability and % area of the main peak was plotted against time for each sample to compare the thermostability of POPC and PC* nanodiscs at different temperatures. SEC-HPLC analytical data of pooled fractions are shown in
Nanodiscs were prepared from GDGT by first drying thirty microliters of 42 nM GDGT lipids in 13×100 mm borosilicate tubes placed in a vacuum desiccator overnight. PC* lipid was dried in parallel. Dried GDGT lipid and dried PC* lipid each were reconstituted in 100 mM Na-cholate+100 mM NaCl according to Table 4. Each tube was vortexed for 30-60 seconds, then sonicated in an 80-100 degrees F. water bath for 15 minutes. Vortexing and sonication was repeated for three cycles with a 10 minute incubation period at room temperature before the last cycle. The tubes were then cooled to room temperature, and the lipids were mixed with MSP and buffer without cholate, then incubated at room temperature for 20 minutes with intermittent mixing by hand. Samples were then cleared of detergent via the addition of AMBERLITE® XAD-2 beads (Rohm and Haas Co.), followed by 5 hours of incubation, and removal of the beads via centrifugation and filtration. The nanodiscs were then subject to thermostability testing.
Assembly of the thermostable nanodisc with an embedded vaccine antigen (e.g., microbial protein such as a viral envelope protein) involves mixing the protein of interest (vaccine antigen) with the membrane scaffolding protein(s) (MSP) and the thermostable phospholipids (e.g., that contain ether linkages) in an aqueous medium under conditions that promote self-assembly of the nanodiscs. Initially, the components are mixed together in an aqueous media containing a detergent, and then the detergent is removed. The nanodiscs then spontaneously assemble, with the antigen protein embedded in a bilayer of the phospholipids. In the assembled nanodisc, the antigen substantially retains its native conformation; the conditions attendant to mixing (including detergent exposure and temperature, even elevated temperatures), detergent removal, filtration, and assembly incubation do not substantially induce denaturing of the vaccine antigen protein.
The process of loading a nanodisc with a membrane glycoprotein (antigen) is similar to that of assembling empty nanodiscs. The protein of interest (e.g., Ebola GP) is first solubilized in a suitable detergent and then added to the disc reconstitution mixture—the mixture of phophoplipids, cholate and membrane scaffold protein (See, Example 4). The microbial protein (e.g., viral envelope protein such as Ebola GP) and the disc reconstitution mixture (phospholipids and MSP) is incubated for about 30 minutes to about an hour to ensure complete mixing. Detergent removal with the help of, for example, AMBERLITE® XAD-2 beads (Rohm & Haas Co.) initiates self-assembly, and the microbial protein is simultaneously self-assembled into the nanodisc—embedded in the bilayer of thermostable phospholipids.
Several key factors responsible for efficient incorporation of a membrane protein target into nanodiscs are to be considered, including—target solubilization detergent, lipid:MSP ratio and detergent removal rate. Detergents such as, but not limited to, ocytlglucoside, dodecyl maltoside, sodium cholate, TRITON® X-100, CHAPS and Fos-choline will be screened to identify conditions that best extract and solubilize monomeric GP from the viral membrane. A combination of size exclusion chromatography and SDS PAGE will be used to evaluate different solubilization conditions.
Depending on the type of lipid and MSP used, nanodiscs may require a particular ratio of phospholipids:MSP during formation for a complete assembly. When a microbial protein antigen is assembled into a nanodisc, the number of lipid molecules it will displace from the nanodisc is not known a priori. Following the identification of a suitable detergent for solubilization, the optimal phospholipid:MSP ratio for microbial protein incorporation would be empirically determined by assembling the protein at different phospholipid:MSP ratios, and identifying the ratio that results in a homogeneous SEC chromatogram.
A microbial protein may self-aggregate as the concentration of solubilizing detergent drops below its critical micellar concentration. Protein incorporation into nanodiscs depends on formation of correct contacts between the phospholipids and the protein as the detergent is being removed from the disc reconstitution mixture. Therefore, the rate of detergent removal is also a factor governing the efficiency of incorporation. Different weight ratios of detergent removal beads (e.g., AMBERLITE® beads) to total detergent used during nanodisc assembly will be used to perform assembly, and the efficiency of incorporation will be determined by comparing the amount of microbial protein (e.g., viral envelope protein) in the assembly mixture and the final nanodisc preparation based on SDS-PAGE and antibody based detection methods such as ELISA and Western blotting.
The approach outlined above been used to optimize incorporation of several membrane proteins into Nanodiscs including recombinant Hemagglutinin from H1N1 and gp-160 from HIV. See, Bayburt, T H et al. (2010) FEBS Letters, 584:1721-7; Bhattacharya, P et al. (2010) J. Virol. 84:361-71; and Nakatani-Webster, E et al. (2015) J. Virol. Methods, 226:15-24.
The loading of vaccine antigen proteins into the nanodisc is illustrated in
The ability of the nanodiscs to generate a protective immune response is tested in a mouse model using challenge with ma-Ebola. Groups of ten mice are inoculated three times with varying doses of vaccine, up to 20 microgram GP content, with two weeks between injections. Nano-VLPs are used as positive control. Anti-GP titers are measured by ELISA. Survival to challenge after 10 days is the key metric of success. If the nanodisc approach proves to be successful, as defined by exhibiting immunopotency at least comparable to that of Nano-VLPs, guinea pig studies are initiated.
A procedure for the assembly of a membrane protein antigen, recombinant hemagglutinin from H1N1 A/New Caledonia/20/99 in this case, into ester and ether-based Nanodiscs and their characterization is described.
A. Assembly of rHA in MSP1D1-POPC Nanodiscs
Assembly of a membrane protein antigen into Nanodiscs involves combining detergent solubilized membrane protein, lipids and membrane scaffold protein (MSP) in specific ratios and incubating the mixture with hydrophobic beads to remove the detergent. Detergent removal initiates self-assembly of the membrane protein of interest into Nanodiscs. Antigen-Nanodiscs may be separated from unincorporated antigen, empty discs and surplus lipid and MSP mixture by the application of appropriate chromatographic purification steps such as affinity chromatography and size exclusion chromatography.
Procedure for rHA Nanodisc Assembly:
1820 nmoles of PC phospholipid (1-palmitoyl-2-oleoyl-sn-glycero-3-phosphocholine, Avanti Polar Lipids; Catalog #850457) were dried under a stream of pure Nitrogen and reconstituted in 36.4 μl of 100 mM sodium-cholate (SAFC; Catalog #S1702-100G; Lot #SLPB3019V)+100 mM NaCl buffer followed by intermittent vortexing and sonication in a 30° C. water bath for 30 minutes.
Separately, 68.5 μl of 598.5 mM β-OG (n-octyl-β-D-glucopyranoside; Anatrace; Catalog #O311; Lot #69360)+300 mM NaCl solution was added to 400 μl of recombinant hemagglutinin (rHA) (Protein Sciences, Catalog #3006; Lot #1368-133) and the rHA detergent mixture was placed on a shaker platform at 4° C. for 1 hour.
Disc reconstitution mixture was prepared by adding 159 μl of 176.6 μM MSP1D1 (BioNanoCon; Lot #150221B), 36.4 μl of 200 mM sodium cholate and 40 μl of 20% (w/v) β-OG to the cholate solubilized lipids. 455 μl of β-OG solubilized rHA was added to the disc reconstitution mixture (DRM). The final volume was adjusted to 728 μl using buffer (50 mM sodium phosphate pH 7.2+150 mM NaCl) and the mixture incubated on ice with gentle shaking for 1 hour. The final concentrations of lipids, sodium cholate, β-OG, MSP1D1 and rHA in the mixture were 2.5 mM, 15.0 mM, 87.5 mM, 38.5 μM and 1.9 μM respectively.
After an hour of incubation, 305 mg of Biobeads SM-2 (BioRad; Catalog #152-3920; Lot #64037853; Exp: 2016 Jan. 26) were added to the mix and the tube was incubated on ice for another 2 hours. Biobeads were rinsed with buffer before use. After 2 hours, Biobeads were removed and rinsed with 400 μl buffer twice. The Nanodisc solution and the wash were combined and filtered through a 0.22 μm filter. The mixture was then purified via SEC. Column used: Superdex 200 Inc. 10/300 GL (GE Healthcare; Code #28-9909-44; Lot #10226065; Exp: 2019 June, ID: 0121). 0.22 μm filtered 50 mM sodium phosphate pH 7.2+150 mM NaCl was used as the running buffer.
The disc assembly process described above results in the formation of rHA monomers, dimers and trimers in Nanodiscs.
SEC fractions from the purification of rHA Nanodiscs were analyzed for their rHA and MSP content using a densitometric analysis of individual SEC fractions on an SDS PAGE gel. Total protein load was normalized to 0.5 μg.
Characterization of rHA Nanodiscs Using SDS-PAGE:
In Vitro Hemagglutination Assay on rHA ND SEC Fractions:
To confirm that rHA in Nanodiscs is active, an in vitro hemagglutination assay was performed. Briefly, 7-two-fold dilutions of SEC fractions B1-B9 were prepared in a 96-wells plate starting at 25 μg/ml. An equal volume of 0.6% chicken red blood cells (Lampire Biological Laboratories; Catalog #7241409; Lot #16K28200) in PBS was added to each well and the contents mixed thoroughly with the help of a pipette. 1×PBS and empty ND show settling of cell suspension indicating the lack of agglutination.
B. Assembly of rHA in 16:0 Ether PC Nanodiscs
Procedure for rHA Nanodisc Assembly:
25 μl of 50 mg/ml 16:0 diether PC (1,2-di-0-hexadecyl-sn-glycero-3-phosphocholine, Avanti Polar Lipids, Catalog #999992, Lot #160DEPC-14) was dried under a stream of pure nitrogen and reconstituted in 35.4 μl of 100 mM sodium-cholate (SAFC; Catalog #S1702-100G; Lot #SLPB3019V)+100 mM NaCl buffer followed by intermittent vortexing and sonication in a 30° C. water bath for 30 minutes.
Separately, 150.4 μl of 598.5 mM β-OG (n-octyl-β-D-glucopyranoside; Anatrace; Catalog #0311; Lot #69360)+300 mM NaCl solution was added to 1050 μl of recombinant hemagglutinin (Protein Sciences, Catalog #3006_H1_NC; Lot #1368-133) and the rHA detergent mixture was placed on a shaker platform at 4° C. for 1 hour.
Disc reconstitution mixture was prepared by adding 103.4 μl of 190.2 μM MSP1D1 (BioNanoCon; Lot #150221B), 58.2 μl of 200 mM sodium cholate and 40.4 μl of 20% (w/v) β-OG to the cholate solubilized lipids. 446 μl of β-OG solubilized rHA was added to the disc reconstitution mixture (DRM). The final volume was adjusted to 842.9 μl using buffer (100 mM sodium phosphate pH 7.4+150 mM NaCl) and the mixture incubated on a shaker platform with gentle shaking for 30 minutes. The final concentrations of lipids, sodium cholate, β-OG, MSP1D1 and rHA in the mixture were 2.1 mM, 18.0 mM, 75.0 mM, 23.3 μM and 1.7 μM respectively.
After an hour of incubation, 760 mg of Amberlite® XAD®-2 (Sigma-Aldrich; Catalog #10357) were added to the DRM and the tube was incubated at 37° C. for 2 hours followed by an hour-long incubation 25° C. After the incubation, Amberlite beads were removed and rinsed with 1 ml buffer. The Nanodisc solution and the wash were combined and filtered through a 0.22 μm filter. The mixture was then purified via SEC. Column used: Superdex 200 Inc. 10/300 GL (GE Healthcare; Code #28-9909-44; Lot #10226065; Exp: 2019-06, ID: 0121). 0.22 μm filtered, 100 mM sodium phosphate pH 7.4+150 mM NaCl was used as the running buffer.
The disc assembly process described above results in the formation of rHA monomers, dimers and trimers in Nanodiscs.
Characterization:
We have shown here that purified recombinant hemagglutinin can be assembled into Nanodiscs using both ester and ether-based lipids, POPC and 16:0 dietherPC respectively. In vitro, hemagglutination analysis shows that rHA in Nanodiscs is functionally active Disc assembly results in formation of all-trimeric, dimeric and monomeric forms of rHA, present in separate fractions of a size-exclusion chromatrography purification run, thus allowing a precise control on the oligomeric state of rHA.
The present disclosure is not limited to the embodiments described and exemplified above, but is capable of variation and modification within the scope of the appended claims.
This application is a continuation-in-part of PCT Application No. PCT/US2016/032703, filed May 16, 2016, which claims priority to U.S. Provisional Application No. 62/162,704, filed May 16, 2015, the contents of which are incorporated by reference herein, in their entirety and for all purposes.
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Number | Date | Country | |
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20180085313 A1 | Mar 2018 | US |
Number | Date | Country | |
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62162704 | May 2015 | US |
Number | Date | Country | |
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Parent | PCT/US2016/032703 | May 2016 | US |
Child | 15813706 | US |