The present invention provides for the intratumoral delivery of immunomodulators. In particular, it provides delivery of co-stimulatory molecules by intratumoral electroporation.
Immunotherapy has recently drawn attention as a forth method following surgery, chemotherapy and radiation therapy for treating tumors. Since immunotherapy utilizes the immunity inherent to humans, it is said that the physical burden on patients are less in immunotherapy than those in other therapies. The therapeutic approaches known as immunotherapies include: cell transfer therapy in which cells such as lymphokine-activated cells, natural killer T-cells or y5T cells obtained, for example, from exogenously-induced cytotoxic T-lymphocytes (CTLs) or peripheral blood lymphocytes by expansion culture using various method are transferred; dendritic cell-transfer therapy or peptide vaccine therapy by which in vivo induction of antigen-specific CTLs is expected; Th1 cell therapy; and immune gene therapy in which genes expected to have various effects are introduced ex vivo into the above-mentioned cells to transfer them in vivo. In these immunotherapies, CD4-positive T cells and CD8-positive T cells have traditionally known to play a critical role.
CD8-positive T cells are major effector cells that are capable of directly destroying tumor cells in vivo and in vitro. These cells are strictly specific to antigen peptides presented by MHC Class 1 molecules. In contrast, antigen specificities of NKT cells are not so strict, and they are considered to be effector cells that show intrinsic immune responses.
CD4-positive T cells are considered to have a fundamental role to regulate anti-tumor immune responses through a plurality of mechanisms although they do not destroy tumors directly. CD4-positive T cells that have recognized a tumor-antigen peptide represented by MHC Class II molecules promote the activation and proliferation of CTL through the interaction with antigen-presenting cells (APCs).
In contrast, CD25-positive/CD4-positive cells (regulatory T cells: Treg) have been shown to inhibit the anti-tumor immune responses and progression of various autoimmune diseases (see US 2003049696 and S. Sakaguchi et al., Immunol. Rev. 182 (2001), pp 18-32). Specifically, since regulatory T cells suppress the activity of cytotoxic CD8-positive T cells through the control of the helper function by targeting CD4-positive T cells, some tumors are considered to utilize this system for their proliferation, thereby avoiding attack of the immune system.
GITR, which has been found as a gene expressed in regulatory T cells (“Tregs”; see S. Sakaguchi et al., Immunol. Rev. 182 (2001), pp 18-32), is a cell surface transmembrane protein receptor and a member of the tumor necrosis factor receptor (TNFR) superfamily. GITR has been shown to be constitutively present on Tregs and activated T cells. GITR binds to another transmembrane protein referred to as GITR ligand (hereinafter referred to as “GITR-L”). Agonistic antibodies against GITR have been shown to abrogate the immunosuppressant activity of regulatory T cells, suggesting that GITRL plays a functional role in regulating the activity of regulatory T cells via GITR (see McHugh et al., Immunity 16 (2002), PP 311-23). Similarly, other co-stimulatory molecules such as CD137, CD134, CD40L, CD27, etc. also function to stimulate immunity.
In vivo electroporation is a gene delivery technique that has been used successfully for efficient delivery of plasmid DNA to many different tissues. Studies have reported the administration of in vivo electroporation for delivery of plasmid DNA to B16 melanomas and other tumor tissues. Systemic and local expression of a gene or cDNA encoded by a plasmid can be obtained with administration of in vivo electroporation. Use of in vivo electroporation enhances plasmid DNA uptake in tumor tissue, resulting in expression within the tumor, and delivers plasmids to muscle tissue, resulting in systemic expression of secreted proteins, such as cytokines (see, e.g., U.S. Pat. No. 8,026,223).
It has been shown that electroporation can be used to transfect cells in vivo with plasmid DNA. Recent studies have shown that electroporation is capable of enhancing delivery of plasmid DNA as an antitumor agent. Electroporation has been administered for treatment of hepatocellular carcinomas, adenocarcinoma, breast tumors, squamous cell carcinoma and B16.F10 melanoma in rodent models. The B16.F10, CT-26, and MC-38 murine syngeneic tumor models has been used extensively for testing potential immunotherapy protocols for the delivery of an immudulatory molecule including cytokines either as recombinant protein or by gene therapy.
Various protocols known in the art can be utilized for the delivery of plasmid encoding a co-stimulatory agonist utilizing in vivo electroporation for the treatment of cancer. The protocols known in the art describe in vivo electroporation mediated cytokine based gene therapy, both intratumor and intramuscular, utilizing low-voltage and long-pulse currents.
Accordingly, what is needed in the art is an electroporation protocol for the delivery of a plasmid encoding a co-stimulatory agonist, such as a GITRL, CD137, CD134, CD40L, and CD27 agonist, that will provide substantially improved results in the regression of cancer tumors, such as melanoma, while also substantially improving the long-term survival rates.
The present invention provides a method for the treatment of malignancies, wherein the administration of a plasmid encoding for a therapeutic co-stimulatory protein, in combination with electroporation has a therapeutic effect on primary tumors as well as distant tumors and metastases.
The present invention provides a method of treating a subject having a cancerous tumor comprising: injecting the cancerous tumor with an effective dose of plasmid coding for a therapeutic protein; and administering electroporation therapy to the tumor, the electroporation therapy further comprises the administration of at least one voltage pulse of about 200 V/cm to about 1500 V/cm over a pulse width of about 100 microseconds to about 20 milliseconds. In certain embodiments, the cancerous tumor is melanoma. In a further embodiment, the plasmid coding for a therapeutic protein is a plasmid coding for a co-stimulatory molecule, and the co-stimulatory molecule can be selected from GITR, CD137, CD134, CD40L, and CD27 agonists. In a further embodiment, the plasmid further encodes at least one immunostimulatory cytokine, which can be selected from IL-12, IL-15, and a combination of IL-12 and IL-15. In certain embodiments the voltage pulse delivered to the tumor is from about 200V/cm to about 1500V/cm.
The present invention provides a method of treating a subject having a cancerous tumor, the method comprising: administering a first treatment at time T1, wherein the first treatment further comprises injecting the cancerous tumor with a first effective dose of plasmid coding for a therapeutic protein and administering a first electroporation therapy to the tumor at time, the first electroporation therapy further comprising the administration of at least one voltage pulse having a duration of about 100 microseconds to about 20 milliseconds; and administering a second treatment at time T2, wherein time T2 is a time later than time T1, wherein the second treatment further comprises injecting the cancerous tumor with a second effective dose of plasmid coding for a therapeutic protein and administering a second electroporation therapy to the tumor at time T2, the second electroporation therapy further comprising the administration of at least one voltage pulse having a duration of about 100 microseconds to about 20 milliseconds. In certain embodiments, the cancerous tumor is melanoma. In a further embodiment, the therapeutic protein is a co-stimulatory molecule, that can be selected from GITR-L, CD137, CD134, CD40L, and CD27 agonists. In another embodiment, the plasmid further encodes at least one immunostimulatory cytokine, chosen from IL-12, IL-15, and a combination of IL-12 and IL-15. In a certain embodiments the voltage pulse delivered to the tumor is from about 200V/cm to about 1500V/cm. In further embodiment, a third treatment is added at time T3, wherein time T3 is a time later than time T2, wherein the third treatment further comprises injecting the cancerous tumor with a third effective dose of plasmid coding for a therapeutic protein and administering a third electroporation therapy to the tumor, the third electroporation therapy further comprising the administration of at least one voltage pulse having a duration of about 100 microseconds to about 20 milliseconds. Certain embodiments involve injecting an effective dose of plasmid encoding for a therapeutic protein into the cancerous tumor of the subject; and administering electroporation to the subject intratumorally using at least one low voltage pulse having a pulse width of about 100 microseconds to about 20 milliseconds and the voltage pulse delivered to the tumor is from about 200V/cm to about 1500V/cm.
The present invention provides a method of treating a subject having a cancerous tumor, the method I comprising: administering a first treatment at time T1, wherein the first treatment further comprises injecting the cancerous tumor with a first effective dose of plasmid coding for a therapeutic protein and administering a first electroporation therapy to the tumor at time, the first electroporation therapy further comprising the administration of at least one voltage pulse having a duration of about 100 microseconds to about 20 milliseconds; administering a second treatment at time T2, wherein time T2 is a time later than time T1, wherein the second treatment further comprises injecting the cancerous tumor with a second effective dose of plasmid coding for a therapeutic protein and administering a second electroporation therapy to the tumor at time, the second electroporation therapy further comprising the administration of at least one voltage pulse having a duration about 100 microseconds to about 20 milliseconds; and administering a third treatment at time T3, wherein time T3 is a time later than time T2, wherein the third treatment further comprises injecting the cancerous tumor with a third effective dose of plasmid coding for a therapeutic protein and administering a third electroporation therapy to the tumor, the third electroporation therapy further comprising the administration of at least one high voltage pulse having a duration of about 100 microseconds to about 20 milliseconds. In certain embodiments, the cancerous tumor is melanoma. In another embodiment, the therapeutic protein is a co-stimulatory molecule, selected from GITR-L, CD137, CD134, CD40L, and CD27 agonists. In a further embodiment, wherein the plasmid encodes at least one immunostimulatory cytokine, selected from IL-12, IL-15, and a combination of IL-12 and IL-15. In a particular embodiment, the voltage pulse delivered to the tumor is from about 200V/cm to about 1500V/cm.
As used herein, including the appended claims, the singular forms of words such as “a,” “an,” and “the,” include their corresponding plural references unless the context clearly dictates otherwise.
All references cited herein are incorporated by reference to the same extent as if each individual publication, patent application, or patent, was specifically and individually indicated to be incorporated by reference.
As used herein, “co-stimulatory molecule” refers to a group of immune cell surface receptor/ligands which engage between T cells and antigen presenting cells and generate a stimulatory signal in T cells which combines with the stimulatory signal (i.e., “co-stimulation”) in T cells that results from T cell receptor (“TCR”) recognition of antigen on antigen presenting cells. Co-stimulatory molecules include, but are not limited to, agonists of GITR, CD137, CD134, CD40L, CD27, and the like.
As used herein, “co-stimulator of T cells activation” refers to the ability of a co-stimulatory ligand to bind and to activate T cells that have been activated via TCR. Co-stimulatory activation can be measured for T cells by the production of cytokines as is well known and by proliferation assays such as are well known and described in the examples. The soluble form of a co-stimulatory molecule which is biologically active also may be tested for binding to the cognate receptor on activated T cells.
As used herein, a soluble form of a co-stimulatory molecule “derived from an antigen presenting cell” refers to a co-stimulatory molecule normally expressed by B cells, macrophages, monocytes, dendritic cells and other such antigen presenting cells, which has been engineered as described herein to render it soluble. Preferred soluble co-stimulatory molecules derived from an antigen presenting cell include any of GITR-L, CD137-L, CD134-L (a.k.a. OX40-L), CD40, CD28. The soluble form of a co-stimulatory molecule derived from an antigen presenting cell retains the ability of the native co-stimulatory molecule to bind to its cognate receptor/ligand on T cells and stimulate T cell activation.
The term “co-stimulatory molecule agonist” includes soluble co-stimulatory molecules and agonists of co-stimulatory molecule binding partners. For example, the binding partner of GITR-L is GITR. Agonists of GITR can include agonistic GITR antibodies, GITR-L polypeptides, including multimeric soluble and transmembrane forms, GITRL mimetics, or other molecules that engage and induce biological activity of GITR.
As used herein, the term glucocorticoid-induced tumor necrosis factor receptor “GITR” ligand (a.k.a. GITR-L, TNFSF18 (tumor necrosis factor (ligand) superfamily, member 18)) refers to a specific molecule associated with this name and any other molecules that have biological function as co-stimulatory molecules that share at least 80% amino acid sequence identity, preferably at least 90% sequence identity, more preferably at least 95% sequence identity and even more preferably at least 98% sequence identity with GITR-L as defined in Swiss Prot Id. no. Q9UNG2).
As used herein, the term “CD137-L” or “agonist of CD137” (a.k.a. 4-1 BB ligand or TNFL9) refers to a specific molecule associated with this name and any other molecules that have biological function as co-stimulatory molecules that share at least 80% amino acid sequence identity, preferably at least 90% sequence identity, more preferably at least 95% sequence identity and even more preferably at least 98% sequence identity with human CD137-L as defined in Swiss Prot Id. no. P41273.
Human CD137-L is a type II membrane protein that contains 254 amino acids (no signal sequence) (see sequence in Swiss Prot Id no. P41273). The protein contains a cytoplasmic domain at residues 1-28, a transmembrane domain at resides 29-49 and an extracellular domain at residues 50-254. The nucleotide sequence of CD137-L (1645 bp) is available in public databases (see Genbank accession no. NM 003811). CD137-L is described by Alderson et al. (1994) Eur J. Immunol. 24(9):2219-27. CD137-L is expressed on antigen presenting cells including B cells, monocytes, and splenic dendritic cells and T lymphocytes. CD137-L interacts with CD137 on activated T cells.
As used herein, the term “CD134-L” or “agonist of CD134” (a.k.a. OX40 ligand or TNRSF4) refers to a specific molecule associated with this name and any other molecules that have biological function as co-stimulatory molecules that share at least 80% amino acid sequence identity, preferably at least 90% sequence identity, more preferably at least 95% sequence identity and even more preferably at least 98% sequence identity with CD134-L, as defined in Swiss Prot Id. no. P23510.
Human CD134-L is a type II membrane protein that contains 183 amino acids (no signal sequence). The protein contains a cytoplasmic domain at residues 1-23, a transmembrane domain at residues 24-50 and an extracellular domain at residues 51-183. The nucleotide sequence of CD134-L (3510 bp, with the coding sequence being 157-708) is available in public databases (see. Genbank accession no. NM_003326.2). CD134-L is described by Godfry et al., J Exp Med. Aug. 1, 1994; 180(2):757-62. CD134-L is expressed by dendritic cells and other APC and binds to CD134, which is present on activated T cells.
As used herein, the term “CD40” (a.k.a. TNFRSF5 or CD40 ligand receptor) refers to a specific molecule associated with this name and any other molecules that have biological function as co-stimulatory molecules that share at least 80% amino acid sequence identity, preferably at least 90% sequence identity, more preferably at least 95% sequence identity and even more preferably at least 98% sequence identity with CD40 as defined in Swiss Prot Id. no. P25942).
The sequence of human CD40 contains 277 amino acids of which 20 amino acids at the N terminus represent the signal sequence (see sequence in Swiss Prot Id no. P25942). A transmembrane domain is located at resides 194-215 and the cytoplasmic domain is located at residues 216-277. The nucleotide sequence of CD40 (1177 bp) is available in public databases (see Genbank accession no. NM_001250). CD40 and various isoforms are described by Tone et al. Proc. Natl. Acad. Sci. U.S.A. 98 (4), 1751-1756 (2001). CD40 is expressed by monocytes and B cells binds to CD40-L (a.k.a. CD40 ligand or CD153) expressed by activated T cells.
As used herein, “CD28” is a type I transmembrane glycoprotein and is a member of the Immunoglobulin family by virtue of its single Ig variable-like extracellular domain which has a MYPPPY (SEQ ID NO: 639) motif required for binding CD80 and CD86 (Peach et al. (1994) J. Exp. Med. 180: 2049-2058). CD28 has a cysteine residue located after the Ig variable-like domain, which is involved in its homodimerization. The protein sequence of CD28 and a nucleic acid encoding a human CD28 are disclosed, for example, in Harper et al. J. Immunol. (1991) 147: 1037-44. The sequence of a human mRNA encoding CD28 also is disclosed in NCBI Accession No. NM_006139, last updated Apr. 19, 2009, for example. The complete protein sequence of a human CD28 also is disclosed in NCBI Accession No. NP_006130.
The term “cancer” includes a myriad of diseases generally characterized by inappropriate cellular proliferation, abnormal or excessive cellular proliferation. Examples of cancer include but are not limited to, breast cancer, colon cancer, prostate cancer, pancreatic cancer, melanoma, lung cancer, ovarian cancer, kidney cancer, brain cancer, or sarcomas. Such cancers may be caused by, chromosomal abnormalities, degenerative growth and developmental disorders, mitogenic agents, ultraviolet radiation (UV), viral infections, inappropriate tissue expression of a gene, alterations in expression of a gene, or carcinogenic agents.
The term “treatment” includes, but is not limited to, inhibition or reduction of proliferation of cancer cells, destruction of cancer cells, prevention of proliferation of cancer cells or prevention of initiation of malignant cells or arrest or reversal of the progression of transformed premalignant cells to malignant disease or amelioration of the disease.
The term “subject” refers to any animal, preferably a mammal such as a human. Veterinary uses are also intended to be encompassed by this invention.
The terms “electroporation”, “electro-permeabilization,” or “electro-kinetic enhancement” (“EP”) as used interchangeably herein refer to the use of a transmembrane electric field pulse to induce microscopic pathways (pores) in a bio-membrane; their presence allows biomolecules such as plasmids, oligonucleotides, siRNA, drugs, ions, and water to pass from one side of the cellular membrane to the other.
The term “biomolecule” as used herein, encompasses plasmid encoded antibodies, antibody fragments, full length immunomodulatory proteins, soluble domains of membrane anchored molecules, fusion proteins, and the like.
Antibodies
The present invention provides an immunotherapeutic approach for reducing the size of a tumor or inhibiting the growth of cancer cells in an individual, or reducing or inhibiting the development of metastatic cancer in an individual suffering from cancer. Therapy is achieved by intratumoral delivery of plasmids encoding various soluble forms of co-stimulatory molecules, or agonists thereof, using electroporation.
Co-stimulatory agonists may be in the form of antibodies or antibody fragments, both of which can be encoded in a plasmid and delivered to the tumor by electroporation.
The term “antibody” as used herein includes immunoglobulins, which are the product of B cells and variants thereof as well as the T cell receptor (TcR), which is the product of T cells, and variants thereof. An immunoglobulin is a protein comprising one or more polypeptides substantially encoded by the immunoglobulin kappa and lambda, alpha, gamma, delta, epsilon and mu constant region genes, as well as myriad immunoglobulin variable region genes. Light chains are classified as either kappa or lambda. Heavy chains are classified as gamma, mu, alpha, delta, or epsilon, which in turn define the immunoglobulin classes, IgG, IgM, IgA, IgD and IgE, respectively. Also subclasses of the heavy chain are known. For example, IgG heavy chains in humans can be any of IgG1, IgG2, IgG3 and IgG4 subclass.
A typical immunoglobulin structural unit is known to comprise a tetramer. Each tetramer is composed of two identical pairs of polypeptide chains, each pair having one “light” (about 25 kD) and one “heavy” chain (about 50-70 kD). The N-terminus of each chain defines a variable region of about 100 to 110 or more amino acids primarily responsible for antigen recognition. The terms variable light chain (VL) and variable heavy chain (VH) refer to these light and heavy chains, respectively.
Antibodies exist as full-length intact antibodies or as a number of well-characterized fragments produced by digestion with various peptidases or chemicals. Thus, for example, pepsin digests an antibody below the disulfide linkages in the hinge region to produce F(ab′)2, a dimer of Fab which itself is a light chain joined to VH-CH1 by a disulfide bond. The F(ab′)2 may be reduced under mild conditions to break the disulfide linkage in the hinge region thereby converting the F(ab′)2 dimer into an Fab′ monomer. The Fab′ monomer is essentially a Fab fragment with the hinge region (see, Fundamental Immunology, W. E. Paul, ed., Raven Press, N.Y. (1993), for a more detailed description of other antibody fragments). A Fab fragment and
Fc fragment are generated by digesting IgG with papain. Papain cleaves in the hinge region just above the residues involved in interchain S—S bonding, resulting in monovalent Fab fragments and the Fc fragment, which includes two constant region fragments, each containing the lower part of the hinge, CH2 and CH3 domains. The constant region fragments of the Fc are stabilized as a dimer though interchain S—S bonding of the lower residues of the hinge region.
Immunoglobulin “Fc” classically refers to the portion of the constant region generated by digestion with papain. Includes the lower hinge which has the interchain S—S bonds. The term “Fc” as used herein refers to a dimeric protein comprising a pair of immunoglobulin constant region polypeptides, each containing the lower part of the hinge, CH2 and CH3 domain. Such “Fc” fragment may or may not contain S—S interchain bridging in the hinge region. It should be understood that an Fc may be from any Ig class and, as such, may include a CH4 domain such as in the case of IgM. Mutant sequences of an Fc are known such as described by Wines et al., J. Immunol. 2000 May 15; 164(10):5313-8 and may be used herein.
While various antibody fragments are defined in terms of the digestion of an intact antibody, one of skill will appreciate that any of a variety of antibody fragments may be synthesized de novo either chemically or by utilizing recombinant DNA methodology. Thus, the term antibody, as used herein also includes antibody fragments either produced by the modification of whole antibodies or synthesized de novo or antibodies and fragments obtained by using recombinant DNA methodologies.
Recombinant antibodies may be conventional full length antibodies, antibody fragments known from proteolytic digestion, unique antibody fragments such as Fv or single chain Fv (scFv), domain deleted antibodies, and the like. Fragments may include domains or polypeptides with as little as one or a few amino acid deleted or mutated while more extensive deletion is possible such as deletion of one or more domains.
An Fv antibody is about 50 Kd in size and comprises the variable regions of the light and heavy chain. A single chain Fv (“scFv”) polypeptide is a covalently linked VH::VL heterodimer which may be expressed from a nucleic acid including VH- and VL-encoding sequences either joined directly or joined by a peptide-encoding linker. See e.g., Huston, et al. (1988) Proc. Nat. Acad. Sci. USA, 85:5879-5883. A number of structures for converting the naturally aggregated, but chemically separated light and heavy polypeptide chains from an antibody V region into an scFv molecule which will fold into a three dimensional structure substantially similar to the structure of an antigen-binding site.
An alternative to the traditional antibody fragments above has been found in a set of unique antibodies produced by the immune systems of camels, llamas, and sharks. Unlike other antibodies, these affinity reagents are composed of only two heavy chains; better yet, a single domain forms the antigen-binding sites for these heavy-chain antibodies. The domains can even be genetically engineered to produce extremely small, very stable single-domain recombinant antibody fragments, called “nanobodies.” Plasmids encoding heavy chain only (VHH), single domain antibodies, and nanobodies are also contemplated for intratumoral delivery by electroporation.
Soluble Agonists
Agonists of co-stimulatory molecules may be soluble molecules such as soluble GITR-L, which comprises at least the extracellular domain (ECD) of GITR-L. Other co-stimulatory molecules will similarly lack transmembrane and intracellular domains, but are capable of binding to their binding partners and eliciting a biological effect. For intratumoral delivery by electroporation, the ECD's will be encoded in an expression vector and will be expressed when delivered to the tumor.
The soluble encoded form of the co-stimulatory molecule may be linked in the expression vector to DNA encoding another protein or polypeptide. Such other polypeptide may be the Fc portion of an immunoglobulin, albumin, or any other type of serum protein or fragment thereof which maintains the solubility of the co-stimulatory molecule. The soluble form of the co-stimulatory molecule may be linked to an immunoglobulin via the heavy and/or light chain, which may be a fragment or a full length heavy or light chain. The immunoglobulin may be an antibody that can target an antigen associated with a cancer cell or tumor. The co-stimulatory molecule may also be expressed on the cell surface of cells, may have the addition of helerologous trimerization domains (e.g. GCN4) or may have point mutations in receptor binding domain that render the ligand more potent (see, e.g., Chattopadhyay et al. (2007) Proc. Natl. Acad. Sci., 104:19452-19457).
The co-stimulatory molecule agonist is delivered as a nucleic acid. Nucleic acid refers to a polynucleotide compound, which includes oligonucleotides, comprising nucleosides or nucleoside analogs that have nitrogenous heterocyclic bases or base analogs, covalently linked by standard phosphodiester bonds or other linkages. Nucleic acids can include RNA, DNA, chimeric DNA-RNA polymers, or analogs thereof. The DNA can be a plasmid expressing a particular co-stimulatory molecule agonist of interest.
The DNA plasmid used for electroporation of encoded co-stimulatory molecules, is one that includes an encoding sequence of a recombinant antigen that is capable of being expressed in a mammalian cell, upon said DNA plasmid entering after electroporation. Preferably, the encoding sequence is a consensus co-stimulatory molecule agonist that elicits an immune response in the target tumor. In some embodiments, the encoding sequence is constructs are optimized for mammalian expression, which can include one or more of the following: including the addition of a Kozak sequence, codon optimization, and RNA optimization. These optimized encoding sequences can be subcloned into various commercially available vectors.
Combination Therapies
It is contemplated that intratumoral electroporation of DNA encoding co-stimulatory agonists can be administered with other therapeutic entities. Table 1 provides possible combinations. Administration of the combination therapies can be achieved by electroporation alone or a combination of electroporation and systemic delivery.
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Other contemplated combination therapies are co-stimulatory agonists combined with: TLR agonists (e.g., Flagellin, CpG); IL-10 antagonists (e.g., anti-IL-10 or anti-IL-10R antibodies); TGFβ antagonists (e.g., anti-TGFβ antibodies); PGE2 inhibitors; Cbl-b (E3 ligase) inhibitors; CD3 agonists; telomerase antagonists, etc. In particular, various combinations of IL-12, IL-15/IL-15Ra, and/or GITR-L are contemplated. IL-12 and IL-15 have been shown to have synergistic anti-tumor effects (see, e.g., Kimura et al. (2000) Cancer Immunol. Immunother. 49:71-77). DNA encoding each molecule can be on separate expression plasmids or combined with appropriate promotors on a single expression plasmid, and delivered to the tumor by various techniques described below.
Electroporation
The devices are contemplated for use in patients afflicted with cancer or other non-cancerous (benign) growths. These growths may manifest themselves as any of a lesion, polyp, neoplasm (e.g. papillary urothelial neoplasm), papilloma, malignancy, tumor (e.g. Klatskin tumor, hilar tumor, noninvasive papillary urothelial tumor, germ cell tumor, Ewing's tumor, Askin's tumor, primitive neuroectodermal tumor, Leydig cell tumor, Wilms' tumor, Sertoli cell tumor), sarcoma, carcinoma (e.g. squamous cell carcinoma, cloacogenic carcinoma, adenocarcinoma, adenosquamous carcinoma, cholangiocarcinoma, hepatocellular carcinoma, invasive papillary urothelial carcinoma, flat urothelial carcinoma), lump, or any other type of cancerous or non-cancerous growth. Tumors treated with the devices and methods of the present embodiment may be any of noninvasive, invasive, superficial, papillary, flat, metastatic, localized, unicentric, multicentric, low grade, and high grade.
The devices are contemplated for use in numerous types of malignant tumors (i.e. cancer) and benign tumors. For example, the devices and methods described herein are contemplated for use in adrenal cortical cancer, anal cancer, bile duct cancer (e.g. periphilar cancer, distal bile duct cancer, intrahepatic bile duct cancer) bladder cancer, benign and cancerous bone cancer (e.g. osteoma, osteoid osteoma, osteoblastoma, osteochrondroma, hemangiorna, chondrornyxoid fibroma, osteosarcoma, chondrosarcoma, fibrosarcoma, malignant fibrous histiocytoma, giant cell tumor of the bone, chordoma, lymphoma, multiple myeloma), brain and central nervous system cancer (e.g. meningioma, astocytoma, oligodendrogliomas, ependymoma, gliomas, medulloblastoma, ganglioglioma, Schwannoma, germinoma, craniopharyngioma), breast cancer (e.g. ductal carcinoma in situ, infiltrating ductal carcinoma, infiltrating lobular carcinoma, lobular carcinoma in situ, gynecomastia), Castleman disease (e.g. giant lymph node hyperplasia, angiofollicular lymph node hyperplasia), cervical cancer, colorectal cancer, endometrial cancer (e.g. endometrial adenocarcinoma, adenocanthoma, papillary serous adnocarcinoma, clear cell) esophagus cancer, gallbladder cancer (mucinous adenocarcinoma, small cell carcinoma), gastrointestinal carcinoid tumors (e.g. choriocarcinoma, chorioadenoma destruens), Hodgkin's disease, non-Hodgkin's lymphoma, Kaposi's sarcoma, kidney cancer (e.g. renal cell cancer), laryngeal and hypopharyngeal cancer, liver cancer (e.g. hemangioma, hepatic adenoma, focal nodular hyperplasia, hepatocellular carcinoma), lung cancer (e.g. small cell lung cancer, non-small cell lung cancer), mesothelioma, plasmacytoma, nasal cavity and paranasal sinus cancer (e.g. esthesioneuroblastoma, midline granuloma), nasopharyngeal cancer, neuroblastoma, oral cavity and oropharyngeal cancer, ovarian cancer, pancreatic cancer, penile cancer, pituitary cancer, prostate cancer, retinoblastoma, rhabdomyosarcoma (e.g. embryonal rhabdomyosarcoma, alveolar rhabdomyosarcoma, pleomorphic rhabdomyosarcoma), salivary gland cancer, skin cancer, both melanoma and non-melanoma skin caner), stomach cancer, testicular cancer (e.g. seminoma, nonseminoma germ cell cancer), thymus cancer, thyroid cancer (e.g. follicular carcinoma, anaplastic carcinoma, poorly differentiated carcinoma, medullary hyroid carcinoma, thyroid lymphoma), vaginal cancer, vulvar cancer, and uterine cancer (e.g. uterine leiomyosarcoma).
The devices and methods of the present embodiment work to treat cancerous tumors by delivering electrical therapy continuously and/or in pulses for a period of time ranging from a fraction of a second to several days, weeks, and/or months to tumors. In a preferred embodiment, electrical therapy is direct current electrical therapy.
The term “electroporation” (i.e. rendering cellular membranes permeable) as used herein may be caused by any amount of coulombs, voltage, and/or current delivered to a patient in any period of time sufficient to open holes in cellular membranes (e.g. to allow diffusion of molecules such as pharmaceuticals, solutions, genes, and other agents into a viable cell).
Delivering electrical therapy to tissue causes a series of biological and electrochemical reactions. At a high enough voltage, cellular structures and cellular metabolism are severely disturbed by the application of electrical therapy. Although both cancerous and non-cancerous cells are destroyed at certain levels of electrical therapy tumor cells are more sensitive to changes in their microenvironment than are non-cancerous cells. Distributions of macroelements and microelements are changed as a result of electrical therapy.
In a single electrode configuration, voltage may be applied for fractions of seconds to hours between a lead electrode and the generator housing, to begin destruction of cancerous tissue. Application of a given voltage may be in a series of pulses, with each pulse lasting fractions of a second to several minutes. In certain embodiments, the pulse duration or width can be from about. Low voltage may also be applied for of a duration of fractions of seconds to minutes, which may attract white blood cells to the tumor site. In this way, the cell mediated immune system may remove dead tumor cells and may develop antibodies against tumor cells. Furthermore, the stimulated immune system may attack borderline tumor cells and metastases.
Various adjuvants may be used to increase any immunological response, depending on the host species, including but not limited to Freund's adjuvant (complete and incomplete), mineral salts such as aluminum hydroxide or aluminum phosphate, various cytokines, surface active substances such as lysolecithin, pluronic polyols, polyanions, peptides, oil emulsions, and potentially useful human adjuvants such as BOG (bacille Calmette-Guerin) and Corynebacterium parvum. Alternatively, the immune response could be enhanced by combination and or coupling with molecules such as keyhole limpet hemocyanin, tetanus toxoid, diptheria toxoid, ovalbumin, cholera toxin or fragments thereof.
U.S. Pat. No. 7,245,963 by Draghia-Akli, et al. describes modular electrode systems and their use for facilitating the introduction of a biomolecule into cells of a selected tissue in a body or plant. The modular electrode systems comprise a plurality of needle electrodes; a hypodermic needle; an electrical connector that provides a conductive link from a programmable constant-current pulse controller to the plurality of needle electrodes; and a power source. An operator can grasp the plurality of needle electrodes that are mounted on a support structure and firmly insert them into the selected tissue in a body or plant. The biomolecules are then delivered via the hypodermic needle into the selected tissue. The programmable constant-current pulse controller is activated and constant-current electrical pulse is applied to the plurality of needle electrodes. The applied constant-current electrical pulse facilitates the introduction of the biomolecule into the cell between the plurality of electrodes. The entire content of U.S. Pat. No. 7,245,963 is hereby incorporated by reference.
U.S. Patent Pub. 2005/0052630 describes an electroporation device which may be used to effectively facilitate the introduction of a biomolecule into cells of a selected tissue in a body or plant. The electroporation device comprises an electro-kinetic device (“EK© device”) whose operation is specified by software or firmware. The EK© device produces a series of programmable constant-current pulse patterns between electrodes in an array based on user control and input of the pulse parameters, and allows the storage and acquisition of current waveform data. The electroporation device also comprises a replaceable electrode disk having an array of needle electrodes, a central injection channel for an injection needle, and a removable guide disk (see, e.g., U.S. Patent Pub. 2005/0052630) is hereby incorporated by reference.
The electrode arrays and methods described in U.S. Pat. No. 7,245,963 and U.S. Patent Pub. 2005/0052630 are adapted for deep penetration into not only tissues such as muscle, but also other tissues or organs. Because of the configuration of the electrode array, the injection needle (to deliver the biomolecule of choice) is also inserted completely into the target organ, and the injection is administered perpendicular to the target issue, in the area that is pre-delineated by the electrodes.
Typically, the electric fields needed for in vivo cell electroporation are generally similar in magnitude to the fields required for cells in vitro. In one embodiment, the magnitude of the electric field range from approximately, 10 V/cm to about 1500 V/cm, preferably from about 300 V/cm to 1500 V/cm and preferably from about 1000 V/cm to 1500 V/cm. Alternatively, lower field strengths (from about 10 V/cm to 100 V/cm, and more preferably from about 25 V/cm to 75 V/cm) the pulse length is long. For example, when the nominal electric field is about 25-75 V/cm, it is preferred that the pulse length is about 10 msec.
The pulse length can be about 10 ps to about 100 ms. There can be any desired number of pulses, typically one to 100 pulses per second. The delay between pulses sets can be any desired time, such as one second. The waveform, electric field strength and pulse duration may also depend upon the type of cells and the type of molecules that are to enter the cells via electroporation.
Uptake of the non-viral delivery vectors of the present invention may also be enhanced by plasma electroporation also termed avalanche transfection. Briefly, microsecond discharges create cavitation microbubbles at electrode surface. The mechanical force created by the collapsing microbubbles combined with the magnetic field serve to increase transport efficiency across the cell membrane as compared with the diffusion mediated transport associated with conventional electroporation. The technique of plasma electroporation is described in Vankov, et al. U.S. Pat. No. 7,923,251 issued Apr. 12, 2011 and Vankov, et al U.S. Pat. No. 8,283,171 issued Oct. 9, 2012. This technique may also be employed in vivo for the transformation of cells. Chalberg, et al (2006) Investigative Ophthalmology & Visual Science 47:4083-4090; Chalberg, et al U.S. Pat. No. 8,101,169 Issued Jan. 24, 2012.
CT-26.WT cells obtained from ATCC (CRL2638) were thawed, and minimally passaged prior to implantation. Adherent CT-26.WT cells were removed from the plate with trypsin and cell viability was determined by AO/PI staining, and live/dead counting was performed using a Cellometer Auto2000 (Nexelcom Biosciences). Cells were resuspended in DPBS at a density of either 1.0×107 live cells/ml or 0.5×107/ml and kept on ice until implantation.
6 week-old female BALB/cJ (stock number 000651) mice purchased from Jackson Laboratories were shaved on both hind flanks one day prior to tumor implantation. Mice were anesthetized with isoflurane until unresponsive to a to pinch test. CT-26.WT cells were drawn into a 1.0 ml sterile syringe using an 18 Ga needle, which was replaced with a 26 Ga needle for implantation. CT-26.WT cell were injected subcutaneously, rostral to the hind flank in a volume of 0.1 ml resulting in implantation of 1.0×106 cells (for primary tumor) or 0.5×106 cells (for contralateral tumor).
Tumor growth was monitored starting 4 days after implantation by measuring long and short axes of tumors with digital calipers. Tumor volume was calculated using the formula for estimating ellipsoid volume (A2×B)/2, where “A” is the short axis and “B” is the long axis. Mice bearing bi-lobed tumors, or tumors implanted deeper than subcutaneous were discarded. When primary tumor volumes reached 40-90 mm3, mice were randomized into cohorts containing similar average tumor volumes. Mice are housed in accordance with AALAM guidelines.
pUMVC3 plasmids (ALDEVERON) for expression of both wild type, as well as recombinant soluble and membrane-bound forms of human GITRL, OX40L, or 4-1 BB (structures illustrated in
Mouse and human GITRL are reported not to cross-react (see, e.g., Bossen et al., (2006) J. Biol. Chem. 281:13964-13971), thus mouse homologs for recombinant human GITRL were constructed for preclinical studies in mice. Mouse GITRL is naturally a dimer. Recombinant mouse GITRL constructs were made as both dimers and trimers using GCN4 multimerization motifs (Harbury, P. B. Nature 371: 80.) The relative binding of dimer and trimer forms to mouse GITR-Fc was compared using a functional ELISA. The trimer form showed higher binding affinity and was used for all further studies (EC50 for dimer, 39.24 uM; EC50 for trimer, 12.38 uM). Substituting the mouse GITRL ECD domain (Genbank Accession #NM_183391) for the human ECD domains in all constructs described above made mouse versions of the SCT forms used in pre-clinical studies. pUMVC3 containing a co-stimulatory molecule agonist (i.e. GITRL) is prepared with an endotoxin-free kit. All plasmid DNA was diluted in sterile injectable saline (0.9%) and stored at −20° C.
Transfection of GITRL plasmids into HEK293 (ATCC) cells with Mirus TranslT-LT1 reagent (Cat. #: MIR 2300). Cell to be transduced are seated at 400,000 cells in a 6-well dish. 24 hours later, Cells were overlaid with 4 μL Mirus and 1 ug DNA). Cell were harvested 4-7 days later for analysis by Western blot, flow cytometry, For activity assays, secreted proteins were harvested from cellular supernatants, and purified using Ni+-resin according to the manufacturers instruction (Novagen)
For Western Blotting, laemmli SDS sample buffer (Alfa Aesar J61337) was added to each sample and boiled at 100 C for 10 minutes and samples were centrifuged. 20 μl of protein+buffer was loaded per well and gel was run at 150 volts for about an hour until the smallest standard reached the bottom of the gel. Gel proteins were transferred to PVDF membranes at 100 volts for 1 hour on ice, rinsed with PVDF 3× with 1×TBST, and then blocked for 1 hour at room temperature on a rocker with 5% BSA in TBST. Rinsed membranes were incubated overnight with Anti-NWSHPQFEK Tag antibody, mAb, mouse (Genscript A01732-100) diluted in TBST+5% nonfat dry milk. Blots were incubated for 1 hour at room temperature with 700 labeled anti-mouse secondary antibody (Rockland). Images were analyzed using a LICOR imager.
For flow cytometry, cells were removed from the dish using warm PBS without Ca++ or Mg++. Cells were counted and distributed into tubes with 5×106 cells/tube, washed and resuspended in 100-200 μl FC buffer (5% filtered FBS+0.1% NaN3 in PBS without Ca++ or Mg++). PE-labeled anti-GITRL (clone 109101 R&D systems), isotype control (clone 11711 R&D systems), or anti-FC and corresponding isotype control (Biolegend) were added and incubated on ice for 1 hour. Samples were washed 3 times with FC buffer. In the case where the sample was to be incubated with anti-FC, the cells were first incubated with anti-GITR-FC fusion protein in FC buffer for 1 hour on ice. Cells were analyzed using a Becton-Dickenson FACScan, GUAVA 12HT flow cytometer (Millipore), or LSR-II (Beckman).
When transduced into HEK 293 human cells, proteins from these constructs were synthesized and properly localized to the extracellular space (soluble form) or on the cell surface and detectable with Anti-NWSHPQFEK Tag antibody by Western Blot, and anti-GITRL Ab by flow cytometry. Membrane-bound trimerized recombinant GITRL proteins, when expressed in HEK 293 cells bound to soluble GITR-FC fusion proteins.
Anti human-Fc antibody (Pierce 31125) was added to flat-bottomed 96 well ELISA plates (Costar cat #3690), diluted to 1 μg/ml diluted with PBS, and incubated at room temperature for 1 hour. Wells were washed with 150 μl PBST 3×, decanted and dried. Wells were blocked by adding 150 μl/well Superblock (Scytek AAA999) and incubated at room temperature for 1 hr. After washing, 50 Owen of recombinant human GITR/TNFRSF18 Fc chimeric protein (R&D 689-GR-100) was added at a concentration of 500 ng/ml. Samples were incubated at room temperature for 1 hour, and subsequently washed. The following were added in triplicate: 50 μl of 5000 ng/ml rhGITRL standard Recombinant Human GITR Ligand/TNFSFI8 (R&D 6987-GL-025) diluted fivefold with PBS down to zero; 50 μl of neat HEK 293 culture supernatant (negative control with no gene expression) diluted fivefold with PBS down to zero; and the soluble human GITRL protein, also titrated. Samples were incubated at room temperature for 1 hour and then washed again. 50 μl/well mouse anti human biotinylated hGTIRL antibody (R&D BAM6943) at 500 ng/ml diluted with PBS was added to each well and incubated at room temperature for 1 hour. After washing, 50 μl/well of 1:15000 strepavidin HRP (Abcam 7403) was added. Samples were incubated at room temperature for 1 hour. After washing, 50 ul/well TMB substrate (Pierce cat #34028) was added and samples were incubated for 10 minutes. Reaction was stopped with the addition of 25 μl/well H2SO4. Optical density was determined using microplate reader set to 450 nm, with wavelength correction set to 540 or 570 nm. The concentration of GITRL in culture supernatants was determined by conventional ELISA using anti-GITRL antibody for binding and detection, and a GITRL protein standard (R&D 6987-GL-025)
Soluble GITRL4 and GITRL-SCT-Fc proteins bind to GITR-FC fusion protein in an ELISA with greater than a 2-fold higher affinity than that of commercially available GITRL protein ((R&D 6987-GL-025; Table 3), and a greater than 2-fold higher specific activity (activity units per ng;
GITRL plasmids were transduced into HEK 293 human cells together with plasmids encoding firefly luciferase under the control of an NFkB-driven promoter (Promega). The plasmid expressing the human GITR gene (Origene), and a plasmid expressing Renilla luciferase were under the control of a constitutive CMV promoter (Promega; control for transduction variability). After 48 hours after transfection, cells were lysed and analyzed for both firefly and Renilla luciferase activity using a Dual Luciferase assay kit (Promega, E1910). Soluble GITRL proteins stimulated GITR signaling to NFkB in a reporter cell line system (
Soluble GITRL proteins were purified from HEK 293 culture supernatants in serum-free conditions using Ni+-Resin as per the manufactures instructions (Novagen). Purified proteins were normalized by A280 absorbance and by ELISA. Molar equivalents of protein were added to engineered Jurkat cells expressing human GITR and an NF-kB-driven secreted luciferase (GITR potency assay, Promega CS184002). A dose response was measured for each protein and compared with commercially available soluble human GITRL (R&D systems). Assay was carried out as per the manufactured instruction with and without the addition of cross-linking antibodies: Anti-HA for R&D GITRL standard (R&D Systems) and Anti-NWSHPQFEK Tag (Genscript) for our GITRL proteins.
Cell surface GITRL proteins were also tested in the GITR potency assay (Promega CS184002) by adapting the assay protocol to co-culture stimulation. HEK 293 cells were transduced with plasmids encoding cell surface GITRL proteins were removed from the dish with PBS-Mg++-Ca++ after 4 days in culture, and plated in a serial dilution from 100,000 down to 1 cell/well in flat bottom 96-well tissue-culture trays (Corning) and left overnight to adhere to substrate. Thaw and use Jurkat cells (Promega CS184002) were overlaid according to the manufacturer instruction onto GITRL-expressing HEK 293 cells and co-cultured for 7 hours. Supernatants were removed from co-culture and luciferase activity was measured as described in the standard protocol (Promega GITR Potency Assay) using a BioTek luminometer. Results were compared with untranfected cells as a negative control, and with soluble R&D GITRL as a positive control for each experiment.
Soluble GITRL4 and GITRL-SCT-FC had greater than 3-fold and 10-fold better potency in this GITR activity assay, respectively, than did commercially available human GITRL (R&D Systems). Cell surface GITRL also showed strong activation when co-cultured with Jurkat reporter cells in GITR potency assay (
Primary human Pan T cells (Allcells, PB009-1) were plated in wells coated overnight with anti-CD3 (OKT3 10 ug/ml) alone or in combination with soluble anti-CD28 (15E8, I ug/ml) or culture supernatants from HEK 293 cells with and without prior transfection with soluble GITRL. Cell were cultured in RPMI+10% FBS for 4 days. Un-stimulated control cells were plated in RPMI+10% FBS in parallel.
For cell surface binding, cells that had been stimulated with anti-CD3 and anti-CD28 were washed with FC buffer (5% filtered FBS+0.1% NaN3 in PBS without magnesium or calcium), on ice. Cells were incubated with or without HEK 293 culture supernatants for 1 hour on ice. After washing in FC buffer, cells were incubated with conjugated antibodies: FITC-conjugated-StrepTAG II antibody (GenScript A10736-100), FITC-conjugated isotype control (Invitrogen GM4992), PE-conjugated human GITR antibody. Cells are washed with FC buffer and analyzed by flow cytometry as described above.
For proliferation assay, duplicate wells of stimulated cells or un-stimulated controls were stained with AO/PI vital staining solution (Nexcelom CS2-0106-5ML), and counted on a Cellometer Auto 2000 4 days after stimulation.
For cytokine production assays, CD4+ T-cells and Pan T-cells (Allcells) were costimulated with 0.1, 0.2, or 0.5 ug/ml of anti-human CD3 (Cat #: 100207) from Biolegend and soluble agonist GITRL molecules. Anti-human CD28 (Cat #: 102111) was used as a positive control. Costimulated T-cells were incubated for 72 hours at 37° C. before supernatants were collected. The level of human IFN-γ and IL-2 in cell supernatants was measured by R&D ELISA kits (Cat #: DY485-05 and Cat #: DY402-05).
Recombinant soluble GITRL4 bound to the cell surface of stimulated primary human pan T cells.
Addition of culture supernatant from HEK 293 cells transduced with plasmids expressing GITRL4 increase primary human T cell proliferative response to TCR crosslinking with anti-CD3 antibody, but to a smaller extent than anti-CD28 antibodies. Addition of GTRL proteins also increase cytokine production in response to TRC cross-linking,
Collectively, these data indicate that plasmids encoding the recombinant GITRL proteins are expressed when introduced into cells and can bind to and stimulate cell surface endogenous GITR on T cells. Within the tumor microenvironment, stimulation of cell surface GITR on T lymphocytes is predicted to enhance activation of these lymphocytes within the tumor microenvironment and facilitate an immune response against tumor cells.
Mouse recombinant GITRL proteins were expressed in HEK 293 cells and the retention in the cell (those containing TM domains) or secretion into the culture medium was verified by Western Blot. Binding to GITR on the surface of primary mouse splenocytes was verified by flow cytometry using anti-StrepTAG II antibody (Genscript). Further, an increase in stimulation of primary mouse T cells with a sub-optimal dose of anti-CD3 (1452C11) with addition of purified soluble mouse GITRL proteins was observed in both purified CD4+ and CD8+ T cells, and well as in whole splenocytes cultures. In each case, recombinant mouse GITRL showed comparable or better T cell co-stimulatory activity than the GITR agonist antibody, DTA-1 (BXcell 6E0063). For example, in whole splenocytes plated with 0.5 ugs/ml 1452C11 anti CD-3 Ab (Biolegend 100207), DTA-1 had an EC50 of 1.29 uM, mGITRL-SCT-FcIgG2a had an EC50 of 0.473 uM, mGITRL4 had an EC50 of 3.32 uM.
Mice were anesthetized with isoflurane for treatment. Circular plasmid DNA was diluted to 1 ug/ul in sterile 0.9% saline. 50 ul of plasmid DNA was injected centrally into primary tumors using a 1 ml syringe with a 26 Ga needle. Electroporation was performed immediately after injection. Electroporation of DNA was achieved using a BTX ECM 830 square wave electroporator providing 8 pulses of 350 V/cm, 10 msec each spaced 1 second apart. Electroporation was delivered by a Medpulser handle with needles spaced 0.5 cm apart, configured to deliver current uni-directionally from 2 needles to 2 opposing needles. The electroporation needles were inserted into the tumor where tumor size permitted. Treatments were performed on days 0.4, and 7, or days 0 and 4 depending on the study. Following treatment, tumor volume was determined every 2-3 days using digital calipers as described previously. Mice were euthanized when the volume of either the primary or contralateral tumor reached 1000 mm3.
For each experiment, 10-15 mice cohort were electroporated with plasmids encoding recombinant mouse GITRL proteins and compared with a cohort treated i.p with 500 ugs DTA-1 GITR agonist antibody on Day 1 or left untreated.
As compared with untreated mice, tumor volumes for the electroporated tumors were significantly reduced (
Tumors and spleen were excised from sacrificed mice and placed in RPMI+10% FBS. Splenocytes were isolated by pressing spleen though a 70 micron strainer, subjecting them to hypotonic red blood cell lysis (ACK buffer; ThermoFisher). Isolate splenocytes were purified using lympholyte M (Cedarlane) prior to staining. Tumors were dissociated using Gentle-MACS for tumors (Miltenyi tumor dissociation kit 130-096-730, C-tubes, 130-093-237) and homogenized using an Miltenyi gentleMACS™ Octo Dissociator with Heaters (130-096-427). Samples were stored on ice until all samples were ready. Cells were pelleted at 1200 rpm (800×g) for 5 min at 4 C and resuspended in PBS+2% FBS+1 mM EDTA (PFB) and overlaid onto 5 mL of Lympholyte-M (Cedarlane) in 15-mL conical centrifuge tubes. Lympholyte columns were spun in centrifuge at 2000 rpm (1500×g) for 20 min at room temperature with no brake. Lymphocyte layer was transferred to 10 mL of PBF, then centrifuge 1200 rpm (800×g) for 5 min at 4 C. Cell pellets were gently resuspended in 500 uL of PFB with Fc block (BD Biosciences 553142). In 96-well plate, cells were mixed with a solution of AH1-detramer (immudex JG3294-APC), according to the manufacturers instruction and incubated for 10 minutes at room temperature. Antibody staining cocktails containing the following: Anti-CD45-AF488 (Biolegend 100723), anti-CD3-BV785 (Biolegend 100232), Anti-CD4-PE (eBiescience12-0041), anti-CD8a-APC (eBioscience 17-0081), anti-CD44-APC-Cy7 (Biolegend 103028), anti-CD19-BV711 (Biolegend 11555), were added and incubated at room temperature for 30 minutes. Cells were washed 3 times and fixed in PFB with 1% paraformaldehyde for 15 minutes on ice. Cells were washed with PFB and stored at 4′C in the dark. Samples were analyzed on an LSR II flow cytometer (Beckman).
Intratumoral electroporation of GITRL increased AH1-dextramer-binding CD8+CD44+ T cells in the spleen (
RT-PCR was used to measure gene expression changes within the treated tumor. Flash frozen tumors were resuspended in PBS and homogenized using gentle MACS Dissociator (Miltenyl Biotech). The homogenate was then transferred into Trizol (Life Technologies Corp.). Total RNA was isolated according to manufacturer's protocol followed by DNase treatment. 1 ug RNA was used to prepare cDNA (Maxima H Minus First Strand cDNA Synthesis Kit with dsDNase, Thermo Fisher Scientific). RT-PCR was performed using TaqMan® Fast Advanced Master Mix (Thermo Fisher Scientific.) and a CFX96 (Biorad). Relative mRNA levels were normalized to 18s and the cycle number was used to calculate the amount of each product using the 2-ΔΔCT method (Livak et al, Methods, 2001).
Intratumoral electroporation of GITRL decreased Foxp3 gene expression within the treated tumor (
These analyses of T cells from spleens and tumors of treated mice suggest that intratumoral electroporation of plasmid encoding for recombinant GITRL can alter the Treg levels within the treated tumor, and result in an increase in tumor antigen-reactive effector T cells systemically.
In addition to GITRL monotherapy, a combination study was done using the CT26 syngeneic tumor model. pUMVC3 plasmid encoding GITRL4-TM1 was electroporated intratumorally along with pUMVC3 encoding for the p35 and p40 subunits of the IL-12 cytokine (A Daud et al., (2008) J. Clin. Oncol. 26:5896-5903).
A statistically significant decrease in mean tumor volume of the untreated, contralateral tumor was seen as compared with pUMVC3 vector control or pUMVC3-IL12 plasmid alone as measured 6, 8, 11 and 13 days after first EP treatment. In addition, complete tumor regression of the untreated tumors had faster kinetics. For example, 19 days after treatment began, 7/15 mice had completed regressed contralateral tumors while the IL-12 treated cohort had only 1/15. Moreover, an increase in the number of mice with a complete response (CR) on both the primary (treated) and contralateral (untreated) was observed as compared with pUMVC3-IL-12 alone.
These results indicate that combination therapy with GITRL and IL-12 in the tumor microenvironment of the primary (treated) tumor had greater efficacy than did IL-12 alone on an untreated, contralateral tumor.
IL-12, IL-15 and GITRL all have separate effect on stimulation of the immune system. Plasmids encoding IL-12 α and β subunits, IL-15 and IL-15Ra, and recombinant GITRL are electroporated together (on separate plasmids or in a single plasmid) into CT26 tumors in a contralateral tumor model to assess whether the combination of these 5 genes has more efficacy in regressing established tumors in BALB/c mice. Intratumoral electroporation of a single, large plasmid encoding all 5 genes is also tested for efficacy as compared with untreated mice. In addition, testing of these genes in combination and separately is done in a B16F10 contralateral tumor model in C57/BI6 mice. Tumor volumes are measured over time, and the percent of mice with complete response are measured.
Mice are humanely sacrificed by CO2 asphyxiation. Tumors are excised and placed in 50-ml conical tubes containing 10 ml of 10% formalin. The tissue is stained with H&E after fixation, as follows: after fixation in 10% neutral buffered formalin for 6 hours, representative tissue samples are processed into paraffin blocks using a Miles VIP tissue processor (Miles Inc., Mishawaka, Ind.). Briefly, tissues are dehydrated in ascending grades of ethanol, cleared in xylene, and infiltrated in paraffin (Tissue Prep 2; Fisher Scientific). Following embedding, tissues are sectioned on a standard rotatory microtome and 4 mm sections are retrieved from a waterbath and mounted on glass slides. Three sections per tumor are examined. Sections are heat-dried and stained with H&E (Richard-Allen Scientific, Kalamazoo, Mich.) using standard histologic techniques.
Immunohistochemical staining is conducted to examine the tumors for the presence of CD4+ lymphocytes, CD8+ lymphocytes, and blood vessels using the following antibodies: rat anti-mouse CD4, rat anti-mouse CD8 (Ly2), and rat anti-mouse CD31 (PECAM-1), respectively (PharMingen, Cambridge, Mass.). Mice are humanely sacrificed by CO2 asphyxiation. Tumors are excised with scissors and the skin removed, then immediately frozen in a mixture of dry ice and ethanol, and stored at (80° C.). Frozen sections of 5 m are obtained. For immunohistochemical analysis, rat anti-mouse CD4, rat anti-mouse CD8 (Ly2), or rat anti-mouse CD31 (PECAM-1) is applied to tissue sections at a dilution of 1:50 and incubated for 30 minutes, followed by detection with the Vector Elite Rat IgG Peroxidase kit at 2× concentration (15 minutes each in biotinylated anti-rat IgG and ABC complex). Immunostaining is carried out on the Dako autostainer. Sections are analyzed at 400× magnification.
Statistical analysis is performed by ANOVA, Mann-Whitney test, or two-tailed Student's T-test.
The present application is continuation of U.S. patent application Ser. No. 15/542,415 filed Jul. 7, 2017, which is a 371 National Stage entry of International Application No. PCT/US2016/012759 with an international filing date of Jan. 8, 2016, which claims the benefit of priority to U.S. Provisional Patent Application No. 62/126,300, filed on Feb. 27, 2015, and U.S. Provisional Patent Application No. 62/101,850, filed Jan. 9, 2015, the contents of each of which are incorporated herein by reference in their entirety.
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62126300 | Feb 2015 | US | |
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Parent | 15542415 | Jul 2017 | US |
Child | 18105153 | US |