The invention relates to the expression of voltage-gated ion channels in ciliates, such as Tetrahymena. In particular, the invention provides for high levels of expression of voltage-gated ion channels which are correctly folded and embedded in the plasma membrane at high density, thereby providing for membrane preparations with high densities of such voltage-gated ion channels.
Voltage gated ion channels (VGIC) are membrane proteins that regulate a variety of physiological processes by conducting ions across biological membranes. The human genome encodes 143 VGIC family members making it the third largest superfamily of signal-transducing proteins after protein kinases and G-protein coupled receptors (Yu and Catterall (2004)).
VGICs are commonly classified by selectivity for the ion (K+, Na+, Ca2+) that is primarily conducted across the membrane. However, regardless of ion selectivity, VGIC family members share a common structural theme featuring a principal pore-forming alpha (α) subunit. There are four variations of this structural theme: two structural variations are based on domains comprising six transmembrane (TM) segments and two structural variations are based on domains comprising two transmembrane segments (
Voltage gated potassium channels (Kv) are composed of tetramers of the α subunit with each resembling one of the homologous domains of the Cav and Nav channels (Tempel et al. (1987), Pongs et al. (1988)). A number of other ion channel families contain this structural motif including calcium-activated potassium (KCa) channels, cyclic nucleotide-gated (CNG) channels, hyperpolarization-activated cyclic nucleotide-modulated (HCN) channels and transient receptor potential (TRP) channels (Yu et al. (2005)).
The simplest VGIC structurally is exemplified by the inwardly rectifying potassium ion channels (Kir) that are comprised of four subunits, each having two transmembrane segments termed M1 and M2 that are analogous in structure and function to the S5 and S6 TM segments in the six TM segment Nav, Cav and Kv ion channels (Ho et al. (1993); Kubo et al. (1993)). The final structural variation consists of the two pore motif potassium channels (K2P) that link together two M1 and M2 TM segments (Goldstein et al. (1996); Lesage et al. (1996)).
Physiologically, VGICs can be associated with auxiliary subunits that can influence expression of the channel, trafficking to the cell surface plasma membrane and modulation of voltage gating (Isom et al. (1994)) although the α is sufficient to generate functional ion conducting channels in heterologous recombinant expression systems. Trafficking of VGICs to the cell surface where they exert their effect is an important regulated event in human cells that has been linked to disease when proper ion channel distribution is interrupted (McCleskey and Gold (1999); Morello et al. (2000); Valdivia et al. (2002); Manganas et al. (2001a); Manganas et al. (2001b); Rea et al. (2002); Mantegazza et al. (2010)). The α pore-forming subunit can contain various signal sequences, such as ER retention signals, that will prevent export of the channel from the ER and subsequent trafficking to the cell surface (Swanwick et al. (2010); Vacher and Trimmer (2012)). Auxiliary subunits have been shown to associate with the α subunit of ion channels and directly affect the expression levels and cell surface trafficking of the ion channel by masking a subunit ER retention signals (Zhang et al. (2008)).
The varied roles of VGICs in physiological processes, not surprisingly, suggests many therapeutic indications, collectively known as channelopathies, that are associated with aberrant or absent VGIC function. These include conditions affecting neuronal excitability (e.g., pain, epilepsy), heart (e.g., arrhythmias) and muscle contraction (e.g., paralysis). Additionally, VGICs are being investigated as potential targets for therapeutic intervention in autoimmune disease (Judge et al. (2006); Sun and Li (2013)) and cancer where multiple studies have shown VGIC involvement in proliferation, migration and survival of a variety of cancer cells (Fiske et al. (2006)).
Despite significant effort in developing ion channel therapeutics, targeting indications with an estimated market of $24 billion or more, there have been few VGIC modulating drugs approved by the FDA over the last decade (Hogg et al. (2006)). Historically, the majority of ion channel drug development has focused on identifying and developing small molecule modulators. Small molecule drug discovery is typically carried out by screening compound libraries using analytical outputs that show direct modulation of the target ion channel or, alternatively, a binding event that is further characterized for ion channel effects.
The accepted standard for ion channel functional characterization is electrophysiology that allows real time kinetic and pharmacological analysis of the effects of drug molecule candidates. While electrophysiology is the most detailed analytical tool available for ion channel functional modulation and is key in making hit-to-lead candidate determinations, it is resource intensive and has suffered historically from low throughput. However, progress has been made with increasing screening throughput with, for example, platforms that utilize robotic multi-patch clamp configurations (Patchliner®, Nanion Technologies, Munich, DE) or population patch clamp technology (Ion Work® Quattro™, Molecular Devices Corp., Sunnyvale, Calif., USA) as well as the development of screens with high throughput capabilities including flux assays, atomic absorption spectroscopy, and fluorescence and colorimetric based assays. While random compound library screening continues to be a focus in ion channel drug discovery efforts, attempts at rational drug design based on VGIC three-dimensional structural information has been limited by a lack of solved human VGIC structures. A major factor limiting progress on determining human VGIC structure has been the low levels of recombinant VGIC produced in mammalian cell lines (e.g., HEK-293). This, in turn, represents a bottleneck in generating enough starting material to carry out successful purification of a VGIC that yields sufficient material (typically >10-20 mg) to enter, for example, crystallization trials that will ultimately generate crystals of a quality suitable for X-ray diffraction analysis.
While mammalian VGICs are highly hydrophobic, complex proteins, previous studies have shown that they can be purified from native sources in a way that maintains functionality of the purified protein following reconstitution into proteoliposomes. For example, a number of labs in the early to mid 1980's purified voltage-gated sodium ion channels from rat brains (Hartshorne et al. (1983)) and from the electroplax of Electrophorus electricus (Miller et al. (1983)), and were able to reconstitute functional activity from purified components (Rosenberg et al. (1983); Talvenheimo et al. (1984); Tamkun et al. (1984); Trainer et al. (1993)). More recently, a structure for a voltage-gated sodium channel from Arcobacter butzleri has been solved to 3.2 Å resolution (Payandeh et al. (2012)). Taken together, these results suggest that solving the crystal structure of human VGICs should be feasible if a source of recombinant protein is available for purification of the ion channel.
An important consideration of small molecule development, whether it is from rational design or random screening, is the specificity a potential drug has for a target. With respect to VGICs, this has been particularly challenging as many ion channels belong to families with closely associated members having high levels of homology, particularly within pore-forming domains where many ion channel blockers exert their effect, but nonetheless have significantly different physiological roles. For example, the sodium channel isoforms Na(v)1.7, Na(v)1.8 and Na(v)1.9 have been identified as targets in nociceptor neurons whose modulation ameliorates different pain states. However, strict counter screens are required to characterize potential modulators of these channels for effects on other Nav family members, such as Nav1.5, which is primarily found in cardiac muscle and is responsible for the initial upstroke of the action potential in an electrocardiogram (Zimmer and Surber (2008)).
An obvious alternative to small molecule promiscuity is the development of biologics such as monoclonal antibodies (mAbs) that have high levels of specificity. Despite the appeal of this approach and significant efforts in developing ion channel mAb drug candidates, there has been even less success than there has been in identifying bona fide small molecule drug candidates. There are several challenging aspects of developing modulating ion channel mAbs that are likely the cause of the paucity of success in this endeavor. The first challenge is that, despite the large mass (>150 kDa) of many of the Nav, Cav and Kv VGICs, the targeted extracellular loops, where mAbs are most likely to elicit a modulating effect, are comparatively small and not highly immunogenic, thus hampering immunization efforts. The second challenge is the lack of suitable antigen sources for either immunization programs or antibody screening efforts. Attempts at generating ion channel mAbs via immunization have mostly relied on DNA-based antigens, whole cell or membrane fractions of recombinant mammalian cell lines expressing VGICs, or peptide-based antigens that preferably mimic a targeted extracellular loop structure. Each of these approaches has drawbacks that have thus far contributed to the difficulty in generating ion channel mAbs. Firstly, due to toxicity associated with high levels of expression, recombinant mammalian cell lines typically produce low levels of surface localized, functional recombinant VGICs, which significantly diminishes the antigenic load of cell-based immunogens. Furthermore, cell-based immunogens often include many potential antigens derived from the cell itself that are likely to be more abundant and possibly more immunogenic than the recombinant ion channel, and particularly the associated extracellular loops, making it difficult to generate an ion channel antibody titer that is high enough to effectively screen. DNA-based immunogens are likely to produce a protein that is functional without the added non-specific cell associated antigens of cell-based immunogens, however the yield of protein would be expected to be low and the resultant immune response may not be sufficiently robust to generate a mAb titer high enough to identify potential modulators. Peptide-based antigens usually do not suffer from issues of quantity as they can typically be produced via chemical synthesis or robust cell expression systems such as E. coli. However, the physiological relevance of peptide-based antigens, even those that are 3-dimensionally accurate representations of surface loop structures, will always be limited as they lack the context of other molecular determinants associated with the ion channel antigen that may be necessary to generate a high titer of neutralizing mAbs.
Similarly, antibody-screening applications require sufficient levels of physiologically relevant ion channel antigen that will allow high enough resolution to identify binders. Current mammalian cell-based sources of ion channel antigen and peptide-based antigens are inadequate to enable such screens for the reasons mentioned above.
Clearly, a source of recombinant, physiologically relevant, VGICs at significantly higher cell surface density than is currently available in mammalian cell lines would further enable VGIC drug discovery programs involving rational drug design, small molecule screening and monoclonal antibody development utilizing both immunization and screening strategies.
In one aspect, the invention provides transgenic ciliates comprising a transgene encoding a mammalian voltage-gated ion channel operably joined to regulatory sequences such that the ciliate expresses the voltage-gated ion channel protein.
In some embodiments, the resting membrane potential of the ciliate differs from the resting membrane potential of a healthy native cell in which the voltage-gated ion channel protein is expressed by at least 10 mV, 15 mV or 20 mV. In some embodiments, the resting membrane potential of the ciliate is −15 mV to −40 mV, or −25 mV to −35 mV. In certain embodiments, the resting potential is approximately −30 mV. In some embodiments, the resting membrane potential of the ciliate is less polarized (i.e., closer to zero) than the healthy native cell in which the voltage-gated ion channel protein is expressed.
In some embodiments, the native cell is a mammalian cell selected from the group consisting of a skeletal muscle cell, cardiac muscle cell, smooth muscle cell, astrocyte, neuron, lymphocyte, kidney cell and ovarian cell. In some embodiments, the native cell is an immortalized mammalian cell selected from the group consisting of a HEK cell, CHO cell or Jurkat cell.
In some embodiments, the transgenic ciliate produces glycoproteins including asparagine-linked glycans that lack sialic acid residues. In some embodiments, the ciliate produces glycoproteins that comprise at least one glycan selected from the group consisting of Man5-, Man4- and Man3-GlcNAc2.
In some embodiments, the transgenic ciliate a Tetrahymena species, and in particular embodiments the species is T. thermophila.
In some embodiments, the regulatory sequences comprise a promoter that is activated by a shift to starvation conditions, such as a promoter that regulates the expression of a gene selected from Table 2.
In some embodiments, regulatory sequences comprise an inducible metallothionein promoter, such as a promoter that regulates the expression of a gene selected from Table 3.
In some embodiments, the promoter is endogenous to ciliates, in some embodiments the genus is Tetrahymena and, in particular embodiments the species is T. thermophila.
In some embodiments, the voltage-gated ion channel comprises a pore-forming α subunit, and in some embodiments the voltage-gated ion channel is substantially free of auxiliary sub-units. In some embodiments, the voltage-gated ion channel is selected from the group consisting of sodium, calcium and potassium voltage gated ion channels, and in some embodiments the voltage-gated ion channel is selected from the voltage-gated ion channels in Table 4.
In some embodiments, (a) adenine and thymine nucleotides comprise at least 55% of the nucleotides of the coding sequence of the transgene encoding the mammalian voltage-gated ion channel; or (b) at least 50% of the codons of the coding sequence of the transgene encoding the mammalian voltage-gated ion channel are chosen from the favored codons for expression in the ciliate.
In another aspect, the invention provides methods for producing a recombinant mammalian voltage-gated ion channel in a transgenic ciliate of the invention (described above), by providing the transgenic ciliate and culturing it under conditions which permit or induce expression of the voltage-gated ion channel.
In another aspect, the invention provides lipid bilayers comprising a mammalian voltage-gated ion channel, and tetrahymenol (which is naturally present in the cell membranes of ciliates, including Tetrahymenta spp.).
In some embodiments, the lipid bilayer is substantially free of cholesterol, and in some embodiments the lipid bilayer is substantially free of other mammalian proteins.
In some embodiments, the lipid bilayer is derived from a non-mammalian cell, in some embodiments the cell is a ciliate, in certain embodiments the genus is Tetrahymena and, in particular embodiments the species is T. thermophila.
In some embodiments, the voltage-gated ion channel comprises a pore-forming a subunit, and in some embodiments the voltage-gated ion channel is substantially free of auxiliary sub-units. In some embodiments, the voltage-gated ion channel is selected from the group consisting of sodium, calcium and potassium voltage gated ion channels, and in some embodiments the voltage-gated ion channel is selected from the voltage-gated ion channels in Table 4. In some embodiments, the voltage-gated ion channel comprises glycans selected from the group consisting of Man5-, Man4- and Man3-GlcNAc2.
In some embodiments, the lipid bilayer comprises a cell surface enriched pellicle fraction derived from a transgenic ciliate expressing the mammalian voltage-gated ion channel. In some embodiments.
In another aspect, the invention provides a population of membrane vesicles comprising a lipid bilayer as described above. In some embodiments, at least 50% of the membrane vesicles are oriented right-side-out and are derived from a transgenic ciliate expressing the mammalian voltage-gated ion channel. In some embodiments, greater than 60% of the membrane vesicles have an average diameter of between 30 and 200 nm. In some embodiments, the membrane vesicles were clarified by an extrusion process.
In another aspect, the invention provides compositions comprising at least 75% by weight of a mammalian voltage-gated ion channel, wherein the voltage-gated ion channel is a glycoprotein that lacks sialic acid residues. In some embodiments, the the voltage-gated ion channel comprises at least one glycan selected from the group consisting of Man5-, Man4- and Man3-GlcNAc2. In some embodiments, the voltage-gated ion channel comprises a pore-forming a subunit, and in some embodiments the voltage-gated ion channel is substantially free of auxiliary sub-units. In some embodiments, the composition is substantially free of other mammalian proteins.
In some embodiments, the voltage-gated ion channel is selected from the group consisting of sodium, calcium and potassium voltage gated ion channels, and in some embodiments the voltage-gated ion channel is selected from the voltage-gated ion channels in Table 4.
In some embodiments, the voltage-gated ion channel is reconstituted into a liposome comprising phospholipids to produce a proteoliposome, and in some embodiments, the proteoliposomes have been clarified by an extrusion process.
In another aspect, the invention provides immunogens comprising the transgenic ciliate of the invention, the lipid bilayers of the invention, the populations of membrane vesicles of the invention, or the compositions of the invention as described above and herein.
In another aspect, the invention provides methods for producing antibodies that modulate the activity of a voltage-gated ion channel using the immunogen of the invention.
In another aspect, the invention provides methods for producing therapeutic antibodies using an immunogen of the invention that modulates the activity of the target voltage-gated ion channel.
In another aspect, the invention provides methods for screening compound libraries for small molecules that bind and modulate the activity of mammalian voltage-gated ion channels using the transgenic ciliates of the invention, as described above and herein.
In another aspect, the invention provides methods for screening compound libraries for small molecules that bind and modulate the activity of mammalian voltage-gated ion channels using the lipid bilayers of the invention, the population of membrane vesicles of the invention, or the compositions of the invention, as described above and herein.
These and other aspects of the invention will be apparent to one of ordinary skill in the art from the following detailed description, figures, examples and appended claims.
The following drawings are illustrative of embodiments of the invention and are not meant to limit the scope of the invention as encompassed by the claims.
The patent, scientific and technical literature referred to herein establish knowledge that was available to those skilled in the art at the time of filing. The entire disclosures of the issued U.S. patents, published and pending patent applications, and other publications that are cited herein are hereby incorporated by reference to the same extent as if each was specifically and individually indicated to be incorporated by reference. In the case of any inconsistencies, the present disclosure will prevail.
All scientific and technical terms used herein, unless otherwise defined below, are intended to have the same meaning as commonly understood by one of ordinary skill in the art. References to techniques employed herein are intended to refer to the techniques as commonly understood in the art, including variations on those techniques or substitutions of equivalent or later-developed techniques which would be apparent to one of skill in the art. In addition, in order to more clearly and concisely describe the subject matter which is the invention, the following definitions are provided for certain terms which are used in the specification and appended claims.
As used herein, the term “ciliates” means eukaryotes belonging to the kingdom Chromalveolata, the superphylum Alveolata, and the phylum Ciliophora. Ciliates are complex protozoa characterized by the presence of cilia on their cell surfaces and dimorphic nuclei consisting of a macronucleus and one or more micronuclei. Exemplary genera of ciliates are the Tetrahymena spp. and the Paramecium spp.
As used herein, the term “Tetrahymena spp.” refers to ciliated protozoa in the family of Tetrahymenidae. Exemplary Tetrahymena spp. include, but are not limited to, T. thermophila and T. pyriformis.
As used herein, the term “Paramecium spp.” refers to ciliated protozoa in the family of Parameciidae. Exemplary Paramecium spp. include, but are not limited to, P. tetraurelia, P. aurelia. P. caudatum and P. bursaria.
As used herein, the term “heterologous” means, with respect to two or more nucleic acids, proteins or other biomolecules, that the biomolecules do not occur within the same species in nature. For example, a genetic construct may include a coding sequence which is operably joined to one or more regulatory sequences, and/or to one or more other coding sequences, and these sequences are considered heterologous to each other if they are not found in the same species in nature. Similarly, a protein may include a first polypeptide which is joined to a second polypeptide, and these polypeptides are considered heterologous to each other if they are not found in the same species in nature. Thus, a human voltage-gated ion channel coding sequence and a ciliate promoter sequence are heterologous to each other. Similarly, a human voltage-gated ion channel is heterologous with respect to a ciliate plasma membrane.
As used herein, the term “endogenous” means, with respect to nucleic acids, proteins or other biomolecules, that the molecules occur in nature in a reference cell or species. For example, a genetic construct may include a coding sequence which is operably joined to one or more regulatory sequences, and the regulatory sequences are considered endogenous to each other if they are operably joined to the coding sequence in nature, and/or they are considered endogenous to a species if they are found in the same species in nature. Similarly, a protein that occurs naturally in a specified cell type or species is considered endogenous to that cell or species. Thus, a human voltage-gated ion channel coding sequence and a ciliate promoter sequence are heterologous to each other, but the promoter is endogenous to the ciliate.
As used herein, the term “homolog” means a protein which is evolutionarily-related to and shares substantial structural and functional similarity with a reference protein in a different species (e.g., human and mouse homologs of a voltage-gated ion channel).
As used herein, the term “sequence identity” means the percentage of identical nucleotide or amino acid residues at corresponding positions in two or more sequences when the sequences are aligned to maximize sequence matching, i.e., taking into account gaps and insertions. The comparison of sequences and determination of percent identity between two sequences can be accomplished using a mathematical algorithm. Techniques for determining sequence identity are well known to one skilled in the art. For purposes of this definition, percentage sequence identity can be determined using the sequence comparison algorithm FASTA, version 3.0t78, using default parameters. See also Pearson and Lipman (1988), Proc Natl. Acad. Sci. USA 85(8):2444-8.
As used herein, the term “promoter” means a nucleotide sequence which is capable of binding an RNA polymerase and initiating transcription of a downstream or 3′ coding sequence.
As used herein, the term “transform” means to introduce into a cell a heterologous nucleic acid or nucleic acid analog which replicates within that cell, that encodes a polypeptide sequence which is expressed in that cell (with or without integration into the genome of the cell), and/or that is integrated into the genome of that cell so as to affect the expression of a genetic locus within the genome. The term “transform” is used to embrace all of the various methods of introducing such nucleic acids or nucleic acid analogs, including, but not limited to the methods referred to in the art as transformation, transfection, transduction, or gene transfer, and including techniques such as microinjection, DEAE-dextran-mediated endocytosis, calcium phosphate coprecipitation, electroporation, liposome-mediated transfection, biolistic bombardment, viral-mediated transfection, and the like.
As used herein, the term “transgenic” refers to a cell or organism which has been transformed with a heterologous nucleic acid, causing expression under appropriate conditions of a heterologous protein encoded by the heterologous nucleic acid.
As used herein, the term “vector” means any genetic construct, such as a plasmid, phage, transposon, cosmid, chromosome, virus, virion, etc., which is capable of transferring nucleic acids between cells. Vectors may be capable of one or more of replication, expression, insertion or integration, but need not possess each of these capabilities. Thus, the term includes cloning, expression, homologous recombination, and knock-out vectors. An “expression” vector for a particular heterologous nucleic acid is a vector which can under appropriate conditions cause the encoded protein to be expressed or biosynthesized within the transformed host cell.
As used herein, the term “regulatory sequence” means a DNA transcriptional and translational control sequence such as a promoter, enhancer, polyadenylation signal, terminator, splice signal, and the like, that provide for the expression of a coding sequence as a protein in a host cell.
As used herein, the term “pellicle” means the thin layer supporting the cell membrane in ciliates, protecting them and allowing them to retain their shape, especially during locomotion. The pellicle is formed primarily from closely packed vesicles called alveoli. The term “pellicle preparation” means a preparation including ciliate pellicles and at least some of the associated membrane structures (e.g., alveolar sacs, cilia).
As used herein in connection with membrane vesicles or proteoliposomes, the term “right-side out” means that the terminus of a transmembrane protein which is normally extracellular in native cells expressing the protein is on the outside of a vesicle, liposome or bilayer, and the terminus which is naturally intracellular in native cells expressing the protein is on the inside of the vesicle or liposome.
As used herein, the term “starvation conditions” means conditions of cell culture for ciliates such the cells remain in the G1 phase of the cell cycle and do not divide. Such conditions can be caused by culturing cells in non-nutrient media (i.e., substantially deficient in nutrients generally) or media lacking one or more specific nutrients required for vegetative growth by ciliates. Note that starvation conditions may promote mating reactivity but not subsequent vegetative growth.
As used herein, the terms “increase” and “decrease” mean, respectively, to cause an increase or decrease of at least 5%, as determined by a method and sample size that achieves statistically significance (i.e., p<0.1).
As used herein, the term “statistically significant” means having a probability of less than 10% under the relevant null hypothesis(i.e., p<0.1).
As used herein, the term “clarifying” refers to a process of filtering a heterogeneous population of membrane vesicles and possibly contaminants and debris in order to substantially remove the contaminants and debris and reduce the size heterogeneity of the vesicles by removing larger vesicles. The resulting liquid suspension is more transparent or “clarified.”
As used herein, the recitation of a numerical range for a variable is intended to convey that the invention may be practiced with the variable equal to any of the values within that range. Thus, for a variable that is inherently discrete, the variable can be equal to any integer value within the numerical range, including the end-points of the range. Similarly, for a variable that is inherently continuous, the variable can be equal to any real value within the numerical range, including the end-points of the range. As an example, and without limitation, a variable which is described as having values between 0 and 2 can take the values 0, 1 or 2 if the variable is inherently discrete, and can take the values 0.0, 0.1, 0.01, 0.001, . . . , 0.9, 0.99, 0.999, or any other real values ≧0 and ≦2, if the variable is inherently continuous.
As used herein, the use of singular forms of words, and the use of the singular articles “a,” “an” and “the,” are intended to include and not exclude the use of a plurality of the referenced term unless the context clearly dictates otherwise.
As used herein, unless specifically indicated otherwise, the word “or” is used in the inclusive sense of “and/or” and not the exclusive sense of “either/or.”
The present invention is dependent, in part, upon the discovery that ciliates can be used to express mammalian voltage-gated ion channels at levels which are significantly higher than in other standard expression systems without substantial toxicity to the host cells, and with a high percentage of correctly-folded proteins. This high level of expression leads to a higher density of the VIGCs embedded in the plasma membrane of the ciliates, and allows for the production of membrane fractions and membrane vesicles having higher densities of VIGCs, and higher densities of correctly-folded VGICs, than in other standard expression and purification systems.
Significantly, the invention provides vectors, transformed cells and methods for the production of recombinant mammalian VGICs at sufficiently high levels and of sufficient quality to enable drug discovery programs for both small molecules and large molecule (i.e., biologics). Furthermore, the invention provides compositions of mammalian VGICs in membrane preparations and in purified form derived from the transformed ciliates.
The ciliates which are used for expression of mammalian VIGCs can be any ciliate species within the kingdom Chromalveolata, the superphylum Alveolata, and the phylum Ciliophora. Exemplary genera of ciliates are the Tetrahymena spp. and the Paramecium spp. Exemplary Tetrahymena spp. include, but are not limited to, T. thermophila and T. pyriformis. Exemplary Paramecium spp. include, but are not limited to, P. tetraurelia, P. aurelia, P. caudatum and P. bursaria.
Ciliates are complex protozoa characterized by the presence of cilia on their cell surfaces and dimorphic nuclei consisting of a macronucleus and one or more micronuclei. The ciliates have elaborate membrane systems and devote a large part of their metabolism towards membrane protein production.
In addition to their complex membrane systems, most ciliates can be grown easily and rapidly in the laboratory. For example, Tetrahymena can be cultured at temperatures ranging from 15° C. to 41° C. in a variety of nutritional media, including several peptone-based media; nutritionally complete, totally defined synthetic medium; skim milk-based medium; and, bacterized medium. Cells can be grown in microliter volumes, but with a generation time of 1.5-3 hrs at 30° C., large volume cultures are also quickly established and simply maintained. Although long-term, exclusively vegetative growth generally results in germline senescence (e.g., cultures with decreasing fertility after 12 to 18 months) vegetative clones of interest can be easily frozen in liquid nitrogen for long-term storage (Simon (1982)). For example, although Tetrahymena is usually grown in shaker flasks on the bench top, perfused bioreactors will support cell concentrations as high as 2.2×107 cells/ml (equivalent to a dry weight of 54 g/L, (Hellenbroich et al. (1999)), and industrial media and fermentation processes for growing Tetrahymena in 1200 liter suspensions have been described (Hellenbroich et al. (1999); deConinck et al. (2000)).
Because of their complex biology, ease of growth, and unique genetic structure, Tetrahymena spp. have been in wide use as model systems since the 1950s (Nanney (1980)). The genetics, development, cell physiology, biochemistry, and ultrastructure of Tetrahymena spp. have been intensively investigated (Frankel (2000)) and have yielded numerous insights into a variety of fundamental biological processes, including those with direct relevance to human health. Indeed, the discovery of dynein as the first microtubule-based motor (Gibbons and Rowe (1965)); telomeres and telomerase (Blackburn et al. (1989)); RNA self-splicing (Kruger et al. (1982)); the role of histone acetylation in transcription (Brownell et al. (1996)); and, in vivo functions for histone H1 (Shen and Gorovsky (1996)), histone phosphorylation (Dou and Gorovsky (2000)), and tubulin post-translational modification (Xia et al. (2000)) were all made in Tetrahymena. In recognition of its importance as a model system, the National Institute of General Medical Sciences (NIGMS) and the National Science Foundation (NSF) jointly funded the sequencing of the Tetrahymena macronuclear genome. That effort was completed in late 2003 (to 9× coverage) and is publicly accessible through the Tetrahymena Genome Database (TGD) maintained at Stanford University.
For production of recombinant VGICs, specifically, Tetrahymena has a number of attributes that may allow it to by-pass the limiting factors associated with low expression yields in mammalian expression hosts. For example, in mammalian expression hosts there appears to be an upper limit to how many functional recombinant channels a mammalian cell can localize to its cell surface before those ion channels create a toxic metabolic environment, presumably through the action of functioning channels. No such toxicity is observed in Tetrahymena, thereby allowing the accumulation of many more cell surface recombinant channels. In the case of recombinant VGICs, the reason for this may be partly explained by differences in the resting membrane potential of native human cells and Tetrahymena expression host cells. For example, in human neurons the resting membrane potential is approximately −70 mV, whereas in Tetrahymena the potential is less polarized and is typically −30 mV, and usually −15 mV to −40 mV. Therefore, for VGICs where activation is linked to changes in membrane voltage potential, it is possible that in a human cell line with a more native resting membrane potential, recombinant channels are ‘primed’ for activation where they are able to exert a toxic effect. In Tetrahymena, cell surface localized ion channels would likely be inactive, though still correctly folded, and therefore not exert any metabolic effect.
As noted above the trafficking of VGICs to the cell surface where they exert their effect is an important event in human cells that is regulated by a number of different mechanisms including manipulation of various retention signals by auxiliary subunits. However, ciliates such as Tetrahymena does not encode any obvious orthologs of auxiliary sub units and co-expression of the human beta sub-units is not required for cell surface localization of, for example, Nav1.8 (See
For specific VGIC families, Tetrahymena may be an ideal expression host due to minimal background. For example, although Tetrahymena encodes a large number of cation ion channels, none are annotated voltage-gated sodium channels. Importantly, there is also a lack of biochemical evidence that Tetrahymena harbors sodium VGICs. Therefore the ability to express specific human sodium VGICs in Tetrahymena enables the distinct advantage of characterizing and utilizing those channels in the absence of competing sodium channel ‘noise’.
Many human VGICs are glycoproteins that are modified with asparagine-linked glycans on extracellular loops. Unlike other expression host cells, such as yeast, that can modify proteins with large, hypermannosylated N-linked glycans, Tetrahymena display minimal heterogeneity amongst glycoforms of native glycoproteins that are restricted to Man5-, Man4- and Man3-GlcNAc2 glycans in a roughly 2:2:6 ratio (Taniguchi et al (1985); Weide et al. (2006)). Moreover, recombinant heterologous glycoproteins produced in Tetrahymena can exhibit uniform glycosylation displaying the Man3-GlcNAc2 that represents the tri-mannosyl core common to all eukaryotic N-linked glycans. Therefore, Tetrahymena derived VGICs represent a significantly more appealing protein source for structural analysis by methods such as X-ray crystallography. This in turn provides a powerful enabling technology for rational drug design.
In one aspect, the invention provides methods for the production of mammalian VGICs in ciliates, such as Tetrahymena spp. which can include all or some of the following steps:
1. Optimization of the VGIC Gene Sequence
Ciliates such as Tetrahymena have a slightly different codon usage than that of mammalian cells, such as human cells. Additionally, the Tetrahymena genome is AT rich compared to human or other mammalian genes. Although not necessary, heterologous genes can be optimized for expression in the host ciliate. For example, for human VGIC subunits, which can be greater than 6 Kb in length, optimization of the gene sequence is recommended. to help maintain the fidelity of the gene sequence during cloning manipulations carried out in bacteria. Indeed, cloned VGIC a sub-unit genes often include unwanted mutations (e.g., frameshift mutations) that would render the protein inactive upon expression or result in the production of truncated inactive protein fragments. These mutations presumably arise during cloning manipulations carried out in bacteria because either the gene itself or some expression by-product causes a selective pressure for those genes that have random inactivating mutations. Ciliate (e.g., Tetrahymena spp.) optimized genes that are AT rich (in accordance with a ciliate genome and codon usage table), however, do not result in selection against wild-type sequences during bacterial manipulations as do the same genes that are optimized for expression in, for example, human cells and that are not AT rich. Thus optimizing heterologous VGIC genes with an AT-rich ciliate codon usage table can allow for easier and faster manipulations of the cloned gene product.
2. Construction of VGIC Expression Cassette(s)
A variety of expression cassettes are known in the art which can be used to express heterologous proteins in ciliates (see, for example, Shang et al. (2002); Smith et al. (2004); Weide et al. (2007); WO 2011/107520 by Hartmann and Apelt; U.S. Pat. No. 6,846,481 to Gaertig et al.; U.S. Pat. No. 8,664,374 to Colussi et al.; and U.S Pat. Pub. No. US 2012/0107343 by Clark et al.). Any of these expression systems, or equivalent systems currently existing or developed in the future, can be used to express a heterologous mammalian VGIC protein in a ciliate. Significantly, it is disclosed herein that relatively higher levels of mammalian VGIC expression can be achieved in ciliate cells with relatively less toxicity than achieved in some other standard expression systems. In addition, it is disclosed that a substantial percentage of the VGICs appear to have correct folding than achieved in some other standard expression systems.
In some embodiments, the expression system takes advantage of the natural amplification of copy number of rDNA genes in the macronucleus of ciliates. The ribosomal DNA locus, which is comprised of the 5.7, 18S, and 26S ribosomal RNA coding sequences along with origin of replication (ori) and non-transcribed spacer regions, is present as a single copy in the transcriptionally silent germline micronucleus of Tetrahymena. During macronuclear development, the entire ribosomal DNA locus is excised from the genome and duplicated to form an inverted tandem repeat. Following the addition of telomeres, the ribosomal DNA becomes amplified (relative to bulk DNA) as an autonomously replicating minichromosome reaching ˜9,000 copies per cell in the fully developed, transcriptionally active macronucleus. Amplification is driven by the ribosomal DNA origin of replication. Because the origin of replication for the ribosomal DNA locus of the C-strain of Tetrahymena has a replicative advantage compared with the same origin from B-strains of T. thermophila, it is possible to replace the entire ribosomal DNA complement by introducing a vector containing the C-strain ribosomal DNA locus into B-strain cells at the time that macronuclear development takes place (that is, conjugation). By incorporating a foreign gene into such a ribosomal DNA vector, one can amplify the transgene in parallel with the entire ribosomal DNA locus resulting in high level expression at the RNA and protein levels.
Analysis of expression profiles in the Tetrahymena Gene Expression Database (TGED) of each of the annotated Tetrahymena cation channels shows some consistency in terms of life cycle specific expression (Xiong et al. (2011)). A majority of Tetrahymena ion channels show relatively higher levels of expression during conjugation, a biological event that is preceded by metabolic starvation, a stage at which some ion channels also show high levels of expression. Therefore, in some embodiments, a Tetrahymena promoter derived from a gene that shows higher levels of expression during starvation, is used for expression of recombinant VGICs. Such a “starvation promoter” can act as an inducible promoter that initiates gene expression after the cells are shifted from a nutrient-rich to a nutrient-deprived culture medium. For example, a variety of media can be used to induce starvation-based expression, including but not limited to Dryl's medium (2 mM sodium citrate, 1 mM NaH2PO4, 1 mM Na2HPO4, 1.5 mM CaCl2), NKC medium (0.2% NaCl, 0.008% KCl, 0.12% CaCl2), Tris buffer solution, HEPES buffer solution, or even water. Another potentially significant advantage of induction by starvation is that the starvation media is essentially inert and can be completely devoid of any ion channel substrate (e g., Na+, K+, ligands, etc.), allowing for a very ‘clean’ background in which to produce the ion channel devoid of activity and potentially toxic side effects.
Another option for expression cassettes is to place the VGIC under the control of a metallothionein promoter that induces expression following addition of an inducer to the medium during vegetative growth.
The options of inducing VGIC expression under either starvation or vegetative conditions allows for a customized approach to optimized expression conditions on a target to target basis.
3. Cloning Expression Cassettes into a High-Copy Genetically Stable rDNA Vector
Expression cassettes placing the control of a recombinant mammalian VGIC under the control of either a starvation or metallothionein promoter are cloned en masse into pTRAS, a ribosomal DNA vector (rDNA) described in PCT/US2010/28168. Besides allowing for very high levels of transgene to be maintained in a Tetrahymena cell (up to 18,000 copies per cell), pTRAS also displays higher levels of genetic stability, compared to other rDNA based vectors, when used in conjunction with the selection drug paromomycin.
4. Transformation of Ciliates
Methods for transforming ciliates have been previously described and consist of, among other methods, microinjection (Tondravi and Yao (1986)), electroporation (Gaertig and Gorovsky (1992)) and particle bombardment (Cassidy-Hanley et al. (1997)).
In some embodiments, tungsten particles coated with VGIC rDNA expression vectors are introduced into the ciliate via particle bombardment (Cassidy-Hanley et al. (1997)).
5. Culturing Transformed Ciliates and Inducing Expression of VGIC
The use of ciliates as model organisms for many years has generated multiple descriptions of their growth and maintenance in culture under both non-controlled (for a review see Cassidy-Hanley (2012)) and controlled fermentation conditions (Hellenbroich et al. (1999)).
In some embodiments, Tetrahymena cells can be grown in a variety of media sources from complex peptone-based media to chemically defined media. For example, Tetrahymena is routinely grown in a complex peptone-based media at 30° C.
6. Preparations of Ciliate Membrane Preparations Enriched in VGIC
Following induction of VGIC gene expression, ciliate cells are harvested and processed in several different ways to produce membrane preparations with different constituents, biophysical characteristics and levels of VGIC enrichment. Importantly, preparations are enriched in surface membrane components that harbor cell surface localized recombinant VGIC.
Pellicle (Cell Ghost) Membrane Preparation: Ciliate pellicle fractions are enriched in ciliate cell surface membranes such as the plasma membrane, alveolar sac membranes and may also be associated with dense core granule mucocysts that are attached just beneath the plasma membrane. Pellicle preparations are generated following gentle physical disruption of the cell in a way that maintains cell shape but allows for the removal of cytosolic components and internal membrane structure. Pellicles are recovered following density-gradient fractionation as has been described previously (Nozawa and Thompson (1971))
Membrane Vesicles: Membrane vesicles are more highly processed membrane preparations than pellicles. Whole cells are disrupted by pressure to produce vesicles derived from surface and internal vesicles in either a right-side-out or inside-out orientation. Following vesicle enrichment by differential centrifugation, a two-phase (e.g., PEG-Dextran) partitioning system can be employed to isolate membrane vesicles derived from the plasma membrane in a right-side-out orientation. This method is adapted from one originally developed for plant based material (Yoshida et al. (1983)) although other methods exist to isolate membrane vesicles with a preferred sidedness using, for example, affinity chromatography (Rice and Lindsey (1997)). For example, membrane vesicles derived from Tetrahymena cells expressing VGICs routinely contain a 5-10 fold enrichment of VGICs compared to pellicle preparations. Furthermore, size analysis of ciliate membrane vesicles by dynamic light scattering and negative stain electron microscopy reveals vesicles that are highly homogenous with greater than 60% of the membrane vesicles having an average diameter of between 30 and 200 nm. In some embodiments, greater than 70%, greater than 80%, or greater than 90% of particles have an average diameter in the range of 30 and 200 nm. In some embodiments, greater than 70%, greater than 80%, or greater than 90% of particles have an average diameter in the range of 20-150 nm (see
7. Purification of VGICs from Whole Cell and Cell Surface Ciliate Membrane Preparations
Recombinant VGICs can be purified from both enriched membrane fractions (such as the pellicle fraction) or from whole cells. Purification involves extracting the VGICs from the ciliate membrane with a non-ionic detergent (e.g., TX100, DDM, etc.) and purification with any standard affinity based technique (e.g., dual affinity chromatography steps such as nickel and anti-FLAG antibody resins). During purification steps, detergent and phospholipid additives are typically maintained in buffers to ensure VGIC stability. At the completion of purification, the VGICs can be present in a mixed micelle composed of protein, detergent and phospholipid. The purified protein optionally can be processed further by removal of the detergent and reconstitution into phospholipid-containing liposomes to create proteoliposomes.
The following experimental examples relate to exemplary embodiments of the invention including: (a) the expression in Tetrahymena thermophila of a recombinant form of the gene SCN10A, which encodes the α sub-unit of the human sodium voltage-gated ion channel protein Nav1.8, the generation of membrane products enriched in the α sub-unit of recombinant Nav1.8 protein, and the purification of the α sub-unit of recombinant Nav1.8, (b) the expression in Tetrahymena thermophila of the gene KCNA3 which encodes the human potassium voltage-gated ion channel subunit Kv1.3, and (c) the expression in Tetrahymena thermophila of the gene CACNA1B that encodes the α sub-unit of the human calcium voltage-gated ion channel protein Cav2.2.
These examples illustrate some preferred modes of practicing the present invention, but are not intended to limit the scope of the claimed invention. Alternative materials and methods may be utilized to obtain similar results, and the invention can be used to express many other mammalian voltage-gated ion channels by substituting the appropriate gene for SCN10A, KCNA3 or CACNA1B.
SCN10A Gene Construct Design, Synthesis and Cloning: A synthetic gene was designed wherein the Nav1.8 a subunit coding region of the human SCN10A gene containing a C-terminal dual FLAG (DYKDDDDK) and 10× His epitope tag was optimized for expression in Tetrahymena thermophila. The GC content of the native human gene (NM_006514.2) is 50.69% whereas the GC content of the Tetrahymena optimized gene is 40.25%. The gene was chemically synthesized and cloned into a somatic expression vector, pTIEV5, via PacI and SacI restriction sites engineered into the 5′ and 3′ ends of the synthetic gene, respectively. Transcription of the transgene was under the control of an optimized cadmium-inducible promoter from the metallothionein-5 (MTT5) gene of Tetrahymena thermophila. The expression construct comprising MTT5 promoter, transgene, MTT1 terminator and a neomycin resistance cassette (
Generation of expression strains: B2086 and CU428 T. thermophila strains were grown in modified NEFF medium (0.25% proteose peptone, 0.25% yeast extract, 0.55% glucose, 33 mM FeCl3) at 30° C. One hundred ml of each logarithmically growing culture was centrifuged at 1,100×g for 2 minutes in oil centrifuge tubes, washed in 10 mM Tris pH 7.4 and resuspended in fresh 10 mM Tris pH 7.4 (starvation medium) at a concentration of 200,000-250,000 cells/ml. Cells were incubated for 9-18 hours at 30° C. After starvation, B2086 and CU428 cell cultures were counted and cell concentration was readjusted to 200,000 cells/ml. To induce conjugation, 100 ml of each strain were mixed together in a 4 L flask. Four transformations were performed between 9.5 and 10.5 hours post-mixing using a Biolistic PDS-1000/He Particle Delivery System (BIO-RAD). For each transformation, 20 μl of M17 (BioRad) tungsten bead suspension in sterile water (60 mg/ml) were coated with 4 μg of DNA construct. Fifty ml of conjugating cells were concentrated to ˜1 ml by centrifugation at 1,100×g in oil centrifuge tubes for 2 minutes. Cells were spread on a round 90 mm hardened paper filter (Whatman, Cat. #1450-090) pre-wet with 1.5 ml 10 mM Tris pH 7.4 inside a Petri dish. After the bombardment, the filter with the cells was transferred into a 500 ml flask containing 50 ml NEFF medium. The flasks were incubated on a slow shaker for ˜20 hours at 30° C. At 30 hours post-mixing, 25 ml NEFF medium containing 300 mg/ml paromomycin was added to the 50 ml of cell culture (final paromomycin concentration, 100 mg/ml). Cells were aliquoted into 96 well microplates (150 ml per well). After 3-4 days, the microplates were examined and 5 ml from each of the wells containing paromomycin-resistant cells were transferred into 150 ml NEFF medium containing 100 mg/ml paromomycin on a master 96 well microplate. To identify Nav1.8 expressing clones, 70 drug-resistant clones were grown to ˜5×105 cells/ml and induced for 6 hr with 1 μg/ml of CdCl2. Proteins were resolved by SDS-PAGE and transferred to nitrocellulose membranes before Western blotting. Blots were probed with either an anti-FLAG antibody that recognizes the linear FLAG epitope engineered into the Nav1.8 C-terminus or an anti-PanNav antibody that recognizes a common epitope amongst members of the Nav family of ion channels. Following incubation in primary antibody, blots were probed with secondary goat anti-mouse IgG coupled to HRP for visualization. Once expressing transformants had been identified a time-course was carried out to determine peak expression post-induction.
Nav1.8 cell localization determination: To determine the cellular localization of recombinant Nav1.8, Tetrahymena cells were grown and induced with 2 μg/ml CdCl2 and fixed in 4% paraformaldehyde. Cells were incubated in blocking solution (3% BSA in PBS) for 1-2 hours and then incubated with anti-FLAG antibody (1/100 in blocking solution) for 1 hour at RT, washed and incubated in blocking solution overnight. Cells were subsequently incubated with FITC-conjugated anti-mouse IgG antibody (1/200 in blocking solution) for 1 hour, washed and analyzed by confocal microscopy using an SP5 Leica laser scanning confocal microscope with a 63× oil objective lens. Wild-type control cells were grown, mock induced, fixed, labeled and imaged in the same way as cells expressing Nav1.8.
Nav1.8 is detected at the plasma membrane as well as inside the cell in what appears to be largely perinuclear ER staining indicating that recombinant Nav1.8 trafficks to the Tetrahymena cell surface following translation (
Preparation of surface membrane pellicle fraction enriched in Nav1.8: A 10 ml culture of Nav1.8 expressing cells was started by transferring 0.5-1 ml from a stock tube into NEFF medium containing 100 ng/ml paromomycin (pm). Cultures were grown at 30° C. with 80-100 rpm shaking, 16-36 hrs. One to five ml of the 10 ml culture was transferred into a 1 L flask containing 100 ml NEFF 100 ng/ml pm (1× pm from a 1000× pm stock) and cells incubated for 16-24 hours under the same conditions. Five ml of the 100 ml culture was used to inoculate a 1-2 L NEFF culture and cells incubated for 20-24 hours under the same conditions. When the cell density reached 0.8-1.0×106 cells/ml, gene expression was induced by the addition of CdCl2 to a final concentration of 1 mg/ml. Cells were further incubated at 30° C. with shaking for 6-7 hours. Prior to cell harvesting, 10 sucrose gradients in 50 ml tubes were prepared and kept on ice: bottom layer—15 ml 1.7 M sucrose in Phosphate Buffer, middle layer—15 ml 1 M sucrose in Phosphate Buffer, top layer—10 ml 0.34 M sucrose in Phosphate Buffer. At 4 hours post-induction, the cells were counted and 1 ml samples removed for protein expression analysis. At 4.5 hours post-induction, the cells were harvested by centrifugation: 1,600×g for 5 minutes at room temperature in an RC-5B centrifuge with an F9-4x1000y rotor. The supernatant was decanted and the pellet(s) were resuspended in 500-700 ml 10 mM Tris-HCI pH 7.4 (pre-warmed to 30° C.). Then cells were then spun again under the same conditions. The cell pellet was quickly chilled on ice (less than a minute) and 90 ml ice-cold Phosphate Buffer (0.2 M sodium phosphate pH 7.2, 0.1 M NaCl, 3 mM EDTA) was added. Cells were resuspended by swirling, while the bottle with cells was kept on ice. All the following procedures were performed in the cold room or on ice using ice-cold buffers. The cell density was determined and adjusted to 9-10×106 cells/ml with Phosphate Buffer. Cells were subjected to loose douncing with an “A” grade douncer. Four to six strokes were initially used and the cells examined by microscopy. If more than 10% of the cells still retain cilia a further 2 strokes were used. The cells were harvested by centrifugation (5 minutes at 1,000×g at 4° C.). The cell pellet containing deciliated cells were resuspended in 50 ml Phosphate Buffer supplemented with one tablet of EDTA-free Protease Inhibitors and 200 ml Turbo DNase, in the cold room, just by inverting the tube or using a 10 ml pipette. The cells were then disrupted using a tight douncer (“B” grade) with between 40-100 strokes. The cell lysis/pellicle release was monitored using a microscope. The homogenate was distributed evenly to 10×50 ml tubes containing sucrose gradients (5-7 ml homogenate per gradient, the homogenate was carefully deposited to the top of the gradient, using P1000 pipetteman or disposable plastic pipettes). Gradients were spun in an RTI centrifuge at 2,700×g, 15 minutes at 4° C. The 0.34 M and 1 M sucrose layers were discarded while the whitish band of pellicles at the interface between 1.0 M and 1.7 M sucrose (should be about 80 ml from 10 gradients) was collected. The pellicle containing solution was diluted with an equal volume of phosphate buffer and distributed to three or four 50 ml tubes and spun at 4,080×g, for 20 minutes at 4° C. The supernatant was discarded and the pellets were resuspended in 30-35 ml Resuspension Buffer (20 mM Tris-HCl pH 7.4, 0.1 M NaCl), combined all in one 50 ml tube, and the volume adjusted to 40 ml. The number of pellicles in the 40 ml suspension was determined using a hemacytometer. The pellicles were harvested by centrifugation (4,080×g, 20 minutes at 4° C.). The supernatant was discarded and the pellet frozen in liquid nitrogen and stored, at −80° C.
Preparation of membrane vesicles enriched in Nav1.8: A 1 L culture of cells were grown and induced to express Nav1.8. Cells were harvested by centrifugation and resuspended in 45 or 180 ml of Mucus Secretion Buffer (40 mM Hepes, 2 mM CaCl2 pH 7.4). Mucocyst secretion was induced by the addition of 5 ml dibucaine per/L of culture initially grown. Samples were centrifuged at 2700 g for 10 minutes. The cell pellet was retained and resuspended in 100 ml potassium phosphate buffer (200 mM pH 7.2) containing protease inhibitors. The suspension was microfluidized one time at 1 KPsi and centrifuged at 1000×g for 10 min. The supernatant was collected and further centrifuged at 10,000×g for 20 minutes. The resulting supernatant was further centrifuged at 100,000×g for 1 hour. The 100K×g pellet was resuspended in 5 ml potassium phosphate buffer and stored at −80° C. until further processing. The frozen pellet was thawed and dounce homogenized until no particles were visible. Two grams of resuspended pellet were loaded onto a previously prepared PEG/Dextran two-phase solution (6.6% w/v dextran in 0.2 M potassium phosphate, pH 7.2 and 6.6 PEG w/v dextran in 0.2 M potassium phosphate, pH 7.2). The sample was vortexed for several seconds and allowed to equilibrate at 4° C. for 20 minutes and centrifuged in a clinical centrifuge for 20 min at 4° C. The top layer was harvested and diluted with an equal volume of 1× PBS and centrifuged at 100K×g for 1 h at 4° C. The pellet was resuspended in approximately 100 W of 1× PBS and total protein measured by BCA assay. Total protein concentration was adjusted to 1 mg/ml with 1× PBS. Biophysical characterization of membrane vesicles was carried out by dynamic light scattering (DLS) using a Malvern Zetasizer Nano ZS90 and negative stain electron microscopy (
Purification of Nav1.8: Nav1.8 can be purified from either whole cells or from enriched membrane fractions. Following extraction of Nav1.8, purification via affinity chromatography proceeds in a similar manner regardless of the source material.
Extraction of Nav1.8 from Pellicles: Thaw frozen pellicle, prepared as described above, on ice in 10 ml resuspension buffer (1×PBS, 100 mM choline chloride, 10% glycerol, 20 mM imidazole, pH7.4, EDTA-free Complete protease inhibitor tables) per pellicle preparation derived from a 1 L culture. Homogenize thawed pellicle in a dounce homogenizer (tight handle). Add an equal volume of extraction buffer (resuspension buffer additionally containing 2% TX100 and 0.5% L-a-phosphatidyl choline from egg yolk Type XVI-E) and incubate on a rocking platform at 4° C. for 1 hour. Spin samples at 100,000×g for 1 hour at 4° C. and filter supernatant samples through a 0.45 micron filter. Proceed to Nickel affinity purification.
Extraction of Nav1.8 from Whole Cells: Two liters of Nav1.8 culture was induced with 2 μg/ml CdCl2 for 4 hr and harvested by centrifugation. The resulting cell pellet was resuspended in 100 ml 1× PBS supplied with protease inhibitors at a concentration 1 tablet per 10 ml of cell suspension and Turbo DNase 15 μl/20 ml of PBS. The resulting cell suspension was distributed equally between 4×50 ml conical tubes containing 10 ml of glass beads, washed and chilled on ice prior to sample addition. Cell suspensions were homogenized by vortexing for 10-20 sec pulses keeping samples on ice between pulses. Cell lysis was checked by light microscopy. When there were no visible cell ghosts the homogenates were left on ice for glass beads to settle, following which the homogenate was transferred to fresh 50 ml conical tubes. Cell lysates were spun at 16-20K×g for 30 min. The resulting supernatant was discarded and the pellet was resuspended in 100 ml PBS supplied with protease inhibitors and DNase and spun again. Extraction of Nav1.8 then proceeded as described above for pellicle preparations.
Affinity Purification of Nav1.8: A bed volume, approximately 10% of the extract volume, of nickel sepharose beads twice washed in equilibration buffer (1× PBS, 100 mM choline chloride, 10% glycerol, 20 mM imidazole, 1% TX100, 0.25% phosphatidyl choline, pH7.4) was added to the extract and incubated overnight at 4° C. on a rocking platform. The sepharose beads were collected by centrifugation and washed three times in 7-8 volumes of wash buffer (1× PBS, 100 mM choline chloride, 10% glycerol, 0.1% TX100, 0.025% phosphatidyl choline, EDTA-free protease inhibitors, pH 7.4). Bound protein was eluted in 4 column volumes of elution buffer (1× PBS, 100 mM choline chloride, 10% glycerol, 0.025% TX100, 0.00625% phosphatidyl choline, 250 mM imidazole, EDTA-free protease inhibitors, pH 7.4). The eluted sample was dialyzed overnight at 4° C. in >50 volumes dialysis buffer (1× PBS, 100 mM choline chloride, 10% glycerol, 0.025% TX100, 0.00625% phosphatidyl choline, EDTA-free protease inhibitors, pH 7.4). A bed volume of anti-FLAG M2 affinity gel, approximately 10% of the dialyzed sample, was washed with 2 column volumes low pH buffer (100 mM glycine, 100 mM choline chloride, 150 mM NaCl, 10% glycerol, 0.025% TX100, 0.00625% phosphatidyl choline, pH 3.5) and then twice with 10 column volumes of dialysis buffer. The FLAG affinity resin was added to the dialyzed sample and incubated for 2 hours at 4° C. on a rocking platform. The resin was collected by centrifugation and washed three times with 10 column volumes of dialysis buffer. Bound protein was eluted in 2 column volume elutions of elution buffer (50 mM NaPO4, 150 mM NaCl, 0.025% TX100, 0.00625% phosphatidyl choline, 0.15 mg/ml 3XFLAG peptide, pH 7.4). Elution step was repeated 3 times. Elution fractions were pooled and dialyzed overnight in 100 volumes elution buffer lacking FLAG peptide (50 mM NaPO4, 150 mM NaCl, 0.025% TX 100, 0.00625% phosphatidyl choline, pH 7.4) at 4° C. The dialyzed sample was concentrated approximately 5 fold in a spin column with a 100 kDa MWCO filter. The sample was stored at 4° C. until further processing.
Reconstitution of purified Nav1.8 in Proteoliposome: Liposomes were prepared in the following manner (all steps were carried out in glass vessels): 40 mg of phosphatidyl choline dissolved in chloroform was dried down in a glass tube. The film of dried phosphatidyl choline was resuspended in 1 ml NaPO4 buffer (50 mM NaPO4, 150 mM NaCl, pH 7.4) to produce a 40 mg/ml solution. The solution went through 3 freeze/thaw cycles using liquid nitrogen followed by a 2 minute period in a sonication bath. The entire process was repeated 3 times. Liposomes were stored on ice until further use.
Detergent from affinity purified Nav1.8 was removed by the addition of 0.2 g/ml SM2 biobeads, pre-hydrated in water for 10 minutes. The sample was incubated on ice for 2-3 hours with occasional gentle swirling. The sample was added to pre-prepared liposomes at a ratio of 0.33 ml liposomes: 1 ml protein sample to give a final phosphatidyl choline concentration of 10 mg/ml. The proteoliposome sample was freeze/thawed 3 times in liquid nitrogen followed by a 2 minute sonication bath. The freeze/thaw was repeated once and the entire sample was frozen and stored at −80° C.
Characterization of purified and reconstituted Nav1.8: Following purification and reconstitution into proteoliposomes, Nav1.8 was characterized by a combination of Western blot analysis (as described above) to ensure recovery of the protein, silver stained SDS-PAGE to estimate purity (
KCNA3 Gene Construct Design, Synthesis and Cloning: A synthetic gene was designed wherein the Kv1.3 subunit coding region of the human KCNA3 gene containing a C-terminal dual FLAG (DYKDDDDK) and 10× His epitope tag was optimized for expression in Tetrahymena thermophila. The gene was chemically synthesized and cloned into a somatic expression vector, pTIEV5, via PacI and SacI restriction sites engineered into the 5′ and 3′ ends of the synthetic gene, respectively. Transcription of the transgene was under the control of an optimized cadmium-inducible promoter from the metallothionein-5 (MTT5) gene of Tetrahymena thermophila. The expression construct comprising MTT5 promoter, transgene, MTT1 terminator and a neomycin resistance cassette (
To identify Kv1.3 expressing clones, drug-resistant clones were grown to ˜5×105 cells/ml and induced for 6 hr with 1 μg/ml of CdCl2. Proteins were resolved by SDS-PAGE and transferred to nitrocellulose membranes before Western blotting. Blots were probed with either an anti-FLAG antibody that recognizes the linear FLAG epitope engineered into the Kv1.3 C-terminus or a specific anti-Kv1.3 antibody. Following incubation in primary antibody, blots were probed with secondary goat anti-mouse IgG coupled to HRP for visualization.
Kv1.3 cell localization determination: To determine the cellular localization of recombinant Kv1.3, Tetrahymena cells were grown and induced with 2 μg/ml CdCl2 and fixed in 4% paraformaldehyde. Cells were incubated in the presence of 10 nM fluorescently-tagged Kv1.3 specific toxins Agitoxin-2-TAMRA (AgTX-2-TAMRA) or ShK-TAMRA for 30 minutes at RT. Cells were washed and analyzed by confocal microscopy using an SP5 Leica laser scanning confocal microscope with a 63× oil objective lens. Wild-type control cells were grown, mock-induced, fixed, labeled and imaged in the same way as cells expressing Kv1.3. To determine if the labeling of Kv1.3 expressing cells was specific, cells were also co-incubated with 10 nM ShK-TAMRA in the presence of saturating amounts (100 nM) of either non-labeled Kv1.3 specific Margatoxin (MgTX) or non-specific calcium activated potassium channel blocker Iberiotoxin (IbTX).
CACNA1B Gene Construct Design, Synthesis and Cloning: A synthetic gene was designed wherein the Cav2.2 α subunit coding region of the human CACNA1B gene containing a C-terminal dual FLAG (DYKDDDDK) and 10× His epitope tag was optimized for expression in Tetrahymena thermophila. The gene was chemically synthesized and cloned into a somatic expression vector, pTIEV5, via PacI and SacI restriction sites engineered into the 5′ and 3′ ends of the synthetic gene, respectively. Transcription of the transgene was under the control of an optimized cadmium-inducible promoter from the metallothionein-5 (MTT5) gene of Tetrahymena thermophila. The expression construct comprising MTT5 promoter, transgene, MTT1 terminator and a neomycin resistance cassette (
To identify Cav2.2 expressing clones, drug-resistant clones were grown to ˜5×105 cells/ml and induced for 6 hr with 1 μg/ml of CdCl2. Proteins were resolved by SDS-PAGE and transferred to nitrocellulose membranes before Western blotting. Blots were probed with an anti-Cav2.2 antibody followed by a secondary goat anti-mouse IgG coupled to HRP for visualization.
Cav2.2 cell localization determination: To determine the cellular localization of recombinant Cav2.2, Tetrahymena cells were grown and induced with 2 μg/ml CdCl2 and fixed in 4% paraformaldehyde. Cells were incubated in blocking solution (3% BSA in PBS) for 1-2 hours and then incubated with anti-Cav2.2 antibody (1/100 in blocking solution) for 1 hour at RT, washed and incubated in blocking solution overnight. Cells were subsequently incubated with FITC-conjugated secondary antibody (1/200 in blocking solution) for 1 hour, washed and analyzed by confocal microscopy using an SP5 Leica laser scanning confocal microscope with a 63× oil objective lens.
While this invention has been particularly shown and described with references to preferred embodiments thereof, it will be understood by those skilled in the art that various changes in form and details may be made therein without departing from the spirit and scope of the invention as defined by the appended claims. Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described specifically herein. Such equivalents are intended to be encompassed in the scope of the appended claims.
E. coli
Filing Document | Filing Date | Country | Kind |
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PCT/US15/29290 | 5/5/2015 | WO | 00 |
Number | Date | Country | |
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61988647 | May 2014 | US | |
62016377 | Jun 2014 | US |