CN111254157A - Chimeric antigen receptor targeting humanized CD30 and uses thereof - Google Patents

Chimeric antigen receptor targeting humanized CD30 and uses thereof Download PDF

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CN111254157A
CN111254157A CN202010089152.9A CN202010089152A CN111254157A CN 111254157 A CN111254157 A CN 111254157A CN 202010089152 A CN202010089152 A CN 202010089152A CN 111254157 A CN111254157 A CN 111254157A
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王恩秀
汪晨
张海
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Nanjing Aide Institute Of Immunotherapy Co ltd
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Abstract

The invention relates to a chimeric antigen receptor targeting humanized CD30 and application thereof. In particular, the invention provides a nucleic acid sequence selected from the group consisting of: contains the coding sequence of human DAP12, the coding sequence of T2A, the coding sequence of humanized CD30 single-chain antibody, and the coding sequence of human TREM1 transmembrane and intracellular region which are connected in sequence. The invention also provides a related fusion protein, a vector containing the coding sequence, and applications of the fusion protein, the coding sequence and the vector.

Description

Chimeric antigen receptor targeting humanized CD30 and uses thereof
Technical Field
The invention belongs to the field of chimeric antigen receptors, and particularly relates to a CD 30-targeted chimeric antigen receptor and application thereof.
Background
CD30 is one of the members of the tumor necrosis factor receptor superfamily, and belongs to the type I transmembrane glycoprotein. The normally low level of CD30 is expressed on the surface of activated T, B, NK cells, and is also expressed in lymphocytes infected with viruses (EBV, HCV, HIV), and is frequently over-expressed in diseases such as hodgkin lymphoma and anaplastic lymphoma (ALCL). The research shows that the positive rate of CD30 expression in DLBCL is about 14-37%, while the positive rate in EBV-related DLBCL is 90%, and CD30 is closely related to B cell activation, T cell immune activation, cell proliferation and apoptosis, etc. The intracellular portion of CD30 interacts with multiple members of the TRAF family, mediating both apoptosis in cells via the JNK and p38 signaling pathways and activation of cells via the nfkb signaling pathway. Because CD30 is commonly expressed on the cell surface of lymphomas such as HL, ALCL and DLBCL, currently, CD 30-targeted immune-related therapies are the hot spot in research on lymphoma treatment.
With the development of tumor immunology theory and clinical technology, chimeric antigen receptor T-cell therapy (CAR-T) is one of the most promising tumor immunotherapy at present [ Schmitz M, et al. 10.1155/2010/956304.]. Chimeric Antigen Receptors (CARs) are a core component of CAR-T, CARs can redirect their specificity and reactivity towards selected immune cells, thus conferring on T cells the ability to recognize tumor antigens in an HLA-independent manner, which makes CAR-engineered T cells capable of activating and proliferating, and thus capable of efficiently killing tumor cells, unlike normal T Cell Receptor (TCR) responses, independent of MHC restriction.
The research shows that α chain variable region of TCR is replaced by single chain variable region (scFv) of tumor specific monoclonal antibody, and the scFv is directly connected with T cell signal conducting structure domain to form Chimeric Antigen Receptor (CAR) which is expressed on the surface of T cell, tumor specific antigen can be identified by scFv, activation signal of T cell can be directly generated, T cell activation and proliferation are promoted, and tumor cell is specifically killed.
The invention is directed to novel CARs constructed to target CD30, the invention uses a humanized CD30 (huggn-35) single chain antibody, huggn-35 has high affinity. huggn-35 is a humanized form of monoclonal antibody targeting CD30, and has therapeutic and diagnostic effects on tumors. The invention modifies CAR-T cells and plays a CAR-T cell anti-tumor role aiming at a CD30 target. The invention lays a good foundation for clinical experiments and clinical treatment.
With the accumulation and continued sophistication of the experience of CAR-T cell therapy, there is increasing interest in its use in malignancies. Under the environment, the pace is to be accelerated, and the CAR-T cell therapy is promoted to rapidly advance on the way of treating malignant tumors by applying and developing clinical tests by utilizing the existing work foundation, research and development teams and medical teams.
Disclosure of Invention
In a first aspect, the present invention provides a nucleic acid sequence selected from the group consisting of:
(1) contains the coding sequence of human natural killer activated receptor related protein (DAP12), T2A, anti-CD 30 single-chain antibody, and human medullary triggering receptor (TREM1) transmembrane and intracellular region which are connected in sequence.
In one or more embodiments, the coding sequence for the signal peptide preceding the coding sequence for the anti-CD 30 single chain antibody is as shown in nucleotide sequence 412-474 of SEQ ID NO. 1. In one or more embodiments, the coding sequence of the anti-CD 30 single-chain antibody is shown in the 481-1236 nucleotide sequence of SEQ ID NO. 1. In one or more embodiments, the nucleic acid sequence of human DAP12 is set forth in nucleic acids SEQ ID NO. 1, positions 1-339. In one or more embodiments, the nucleic acid sequence of T2A is as shown in SEQ ID NO 1 at position 355-405. In one or more embodiments, the nucleic acid sequence of the transmembrane and intracellular region of human TREM1 is as shown in SEQ ID NO:1, nucleic acid 1273-1410. In a second aspect, the invention provides a fusion protein selected from the group consisting of:
(2) a fusion protein containing sequentially connected human DAP12, T2A, anti-CD 30 single-chain antibody, human TREM1 transmembrane and intracellular regions and a fusion protein which is formed by substituting, deleting or adding one or more amino acids in a defined amino acid sequence and retains the activity of activated T cells;
preferably, the anti-CD 30 monoclonal antibody is hugGN-35.
In one or more embodiments, the nucleic acid sequence further comprises a coding sequence for a signal peptide prior to the coding sequence for the anti-CD 30 single chain antibody. In one or more embodiments, the amino acid sequence of the signal peptide is as shown in SEQ ID NO:2 amino acids 138-158. In one or more embodiments, the amino acid sequence of the anti-CD 30 single chain antibody is shown as amino acids 161-412 of SEQ ID NO 2. In one or more embodiments, the amino acid sequence of human DAP12 is set forth in SEQ ID NO. 2 amino acids 1-113. In one or more embodiments, the amino acid sequence of T2A is depicted as amino acids 119-135 of SEQ ID NO 2. In one or more embodiments, the amino acid sequence of the transmembrane and intracellular region of human TREM1 is as shown in amino acids 425-469 of SEQ ID NO 2.
In a third aspect, the invention provides a nucleic acid vector comprising a nucleic acid sequence as described herein.
In one or more embodiments, the nucleic acid construct is a lentiviral vector comprising a nucleic acid sequence as described herein, and optionally a selectable marker.
In a fourth aspect, the invention provides a lentivirus comprising a nucleic acid vector as described herein, preferably comprising said lentivirus vector.
In a fifth aspect, the invention provides a genetically modified T cell comprising a nucleic acid sequence as described herein, or comprising a nucleic acid vector as described herein, or infected with a lentivirus as described herein, or stably expressing a fusion protein as described herein.
In a sixth aspect, the invention provides a pharmaceutical composition comprising a genetically modified T cell as described herein.
In a seventh aspect, the invention provides the use of a nucleic acid sequence, fusion protein, nucleic acid vector or lentivirus as described herein in the preparation of an activated T cell.
In an eighth aspect, the invention provides the use of a nucleic acid sequence, fusion protein, nucleic acid vector, lentivirus, or genetically modified T cell, or a pharmaceutical composition thereof, as described herein, in the preparation of a medicament for the treatment of a CD 30-mediated disease.
In one or more embodiments, the CD 30-mediated disease is brain cancer, bladder cancer, breast cancer, cervical cancer, colorectal cancer, liver cancer, kidney cancer, lymphoma, leukemia, lung cancer, melanoma, metastatic melanoma, mesothelioma, neuroblastoma, ovarian cancer, prostate cancer, pancreatic cancer, kidney cancer, skin cancer, thymoma, sarcoma, non-hodgkin's lymphoma, uterine cancer. In one or more embodiments, the CD 30-mediated disease is non-hodgkin's lymphoma, hodgkin's lymphoma.
Drawings
FIG. 1: schematic representation of pELNS-CD30 CAR lentiviral expression vector.
FIG. 2: CD30-CAR structural schematic diagram
FIG. 3: CD30 CAR-T and NTD proliferation profiles
FIG. 4: co-culture of CD30 CAR-T with target cells for cytokine secretion
FIG. 5: CD30 CAR-T killing
Detailed Description
The present invention provides a Chimeric Antigen Receptor (CAR) targeting humanized CD 30. The CAR contains sequentially linked human DAP12, T2A, anti-CD 30 single chain antibody, human TREM1 transmembrane and intracellular domains.
anti-CD 30 single chain antibodies suitable for use in the present invention may be derived from a variety of anti-CD 30 monoclonal antibodies known in the art.
Thus, in certain embodiments, anti-CD 30 chain antibodies suitable for use in the present invention contain a heavy chain that specifically recognizes human CD 30. Optionally, the light chain variable region and the heavy chain variable region may be linked together by a linker sequence. Such single chain antibodies that may be exemplified include, but are not limited to, BerH2, SGN-35, SGN-30, MDX-060, MDX-1401, XmAb2513, AFM 13. In certain embodiments, the monoclonal antibody is huggn-35.
The fusion proteins of the present invention, such as human DAP12, T2A, anti-CD 30 single chain antibody, human TREM1 transmembrane and intracellular domains, etc., may be directly linked to each other or may be linked through a linker sequence. The linker sequence may be one known in the art to be suitable for use with antibodies, for example, a G and S containing linker sequence. Typically, the linker contains one or more motifs which repeat back and forth. For example, the motif may be GGGS, GGGGS, SSSSG, GSGSA and GGSGG. Preferably, the motifs are adjacent in the linker sequence with no intervening amino acid residues between the repeats. The linker sequence may comprise 1, 2, 3, 4 or 5 repeat motifs. The linker may be 3 to 25 amino acid residues in length, for example 3 to 15, 5 to 15, 10 to 20 amino acid residues. In certain embodiments, the linker sequence is a polyglycine linker sequence. The number of glycines in the linker sequence is not particularly limited, and is usually 2 to 20, such as 2 to 15, 2 to 10, 2 to 8. In addition to glycine and serine, other known amino acid residues may be contained in the linker, such as alanine (a), leucine (L), threonine (T), glutamic acid (E), phenylalanine (F), arginine (R), glutamine (Q), and the like.
It will be appreciated that in gene cloning procedures it is often necessary to design appropriate cleavage sites which will introduce one or more irrelevant residues at the end of the expressed amino acid sequence without affecting the activity of the sequence of interest. In order to construct a fusion protein, facilitate expression of a recombinant protein, obtain a recombinant protein that is automatically secreted outside of a host cell, or facilitate purification of a recombinant protein, it is often necessary to add some amino acids to the N-terminus, C-terminus, or other suitable regions within the recombinant protein, for example, including, but not limited to, suitable linker peptides, signal peptides, leader peptides, terminal extensions, and the like. Thus, the amino-terminus or the carboxy-terminus of the fusion protein of the invention (i.e., the CAR) may also contain one or more polypeptide fragments as protein tags. Any suitable label may be used herein. For example, the tag may be FLAG, HA, HA1, c-Myc, Poly-His, Poly-Arg, Strep-TagII, AU1, EE, T7, 4A6, ε, B, gE, and Ty 1. These tags can be used to purify proteins.
The invention also includes a CAR represented by the amino acid sequence of positions 1-469 or a mutant of the CAR represented by SEQ ID NO. 2. These mutants include: an amino acid sequence that has at least 80%, preferably at least 85%, preferably at least 90%, preferably at least 95%, preferably at least 97% sequence identity to the CAR and retains the biological activity (e.g., activating T cells) of the CAR. Sequence identity between two aligned sequences can be calculated using, for example, BLASTp from NCBI.
Mutants also include amino acid sequences having one or several mutations (insertions, deletions or substitutions) in the amino acid sequence shown in positions 1-469 of SEQ ID No. 2 or in the amino acid sequence shown in SEQ ID No. 2, which usually refer to within 1-10, such as 1-8, 1-5 or 1-3, substitutions are preferably conservative substitutions, e.g., conservative substitutions with similarly performing or similar amino acids, which usually do not alter the function of the protein or polypeptide, "similarly performing or similar amino acids" include, for example, families of amino acid residues with similar side chains, which include amino acids with basic side chains (e.g., lysine, arginine, histidine), amino acids with acidic side chains (e.g., aspartic acid, glutamic acid), amino acids with uncharged polar side chains (e.g., glycine, asparagine, glutamine, serine, threonine, tyrosine, cysteine), amino acids with nonpolar side chains (e.g., alanine, valine, leucine, methionine, phenylalanine, tyrosine, amino acids with side chains that are substantially non-polar (e.g., alanine, isoleucine, threonine, tryptophan.
The invention includes nucleic acid sequences encoding the fusion proteins of the invention. The nucleic acid sequences of the invention may be in the form of DNA or in the form of RNA. The form of DNA includes cDNA, genomic DNA or artificially synthesized DNA. The DNA may be single-stranded or double-stranded. The DNA may be the coding strand or the non-coding strand. The invention also includes degenerate variants of the nucleic acid sequences encoding the fusion proteins, i.e., nucleotide sequences which encode the same amino acid sequence but differ in nucleotide sequence.
The nucleic acid sequences described herein can generally be obtained by PCR amplification. Specifically, primers can be designed based on the nucleic acid sequences disclosed herein, particularly open reading frame sequences, and the relevant sequences can be amplified using commercially available cDNA libraries or cDNA libraries prepared by conventional methods known to those skilled in the art as templates. When the sequence is long, two or more PCR amplifications are often required, and then the amplified fragments are spliced together in the correct order. For example, in certain embodiments, the nucleic acid sequence encoding the fusion proteins described herein is as set forth in nucleic acids 1-1410 of SEQ ID NO. 1.
The invention also relates to nucleic acid vectors comprising the nucleic acid sequences described herein, and one or more regulatory sequences operatively linked to these sequences. The nucleic acid sequences of the invention can be manipulated in a variety of ways to ensure expression of the fusion protein (CAR). The nucleic acid vector may be manipulated prior to its insertion into the vector depending on the identity or requirements of the expression vector. Techniques for altering nucleic acid sequences using recombinant DNA methods are known in the art.
The control sequence may be an appropriate promoter sequence. The promoter sequence is typically operably linked to the coding sequence of the protein to be expressed. The promoter may be any nucleotide sequence which shows transcriptional activity in the host cell of choice including mutant, truncated, and hybrid promoters, and may be obtained from genes encoding extracellular or intracellular polypeptides either homologous or heterologous to the host cell. The control sequence may also be a suitable transcription terminator sequence, a sequence recognized by a host cell to terminate transcription. The terminator sequence is operably linked to the 3' terminus of the nucleotide sequence encoding the polypeptide. Any terminator which is functional in the host cell of choice may be used in the present invention. The control sequence may also be a suitable leader sequence, a nontranslated region of an mRNA which is important for translation by the host cell. The leader sequence is operably linked to the 5' terminus of the nucleotide sequence encoding the polypeptide. Any terminator which is functional in the host cell of choice may be used in the present invention.
The nucleic acid sequences of the present invention can be cloned into many types of vectors. For example, it can be cloned into plasmids, phagemids, phage derivatives, animal viruses and cosmids. Further, the vector is an expression vector. The expression vector may be provided to the cell in the form of a viral vector. Viral vector technology is well known in the art and is described, for example, in Sambrook et al (2001, molecular cloning: A Laboratory Manual, Cold Spring Harbor Laboratory, New York) and other virology and molecular biology manuals. Viruses that can be used as vectors include, but are not limited to, retroviruses, adenoviruses, adeno-associated viruses, herpes viruses, and lentiviruses.
Generally, suitable vectors comprise an origin of replication, a promoter sequence, a convenient restriction enzyme site, and one or more selectable markers that function in at least one organism (e.g., WO 01/96584; WO 01/29058; and U.S. Pat. No. 6,326,193).
For example, in certain embodiments, the invention employs a lentiviral vector comprising a nucleic acid sequence as described herein, and optionally a selectable marker.
An example of a suitable promoter is the elongation growth factor-1 α (EF-1 α) promoter sequence Another example of a suitable promoter is immediate early Cytomegalovirus (CMV). however, other constitutive promoter sequences can also be used, including, but not limited to, the simian virus 40(SV40) early promoter, the mouse mammary cancer virus (MMTV), the Human Immunodeficiency Virus (HIV) Long Terminal Repeat (LTR) promoter, the MoMuLV promoter, the avian leukemia virus promoter, the EB virus immediate early promoter, the Rous sarcoma virus promoter, and human gene promoters, such as, but not limited to, the actin promoter, the myosin promoter, the heme promoter, and the creatine kinase promoter.
To assess the expression of the CAR polypeptide or portion thereof, the expression vector introduced into the cells can also comprise either or both of a selectable marker gene or a reporter gene to facilitate identification and selection of expressing cells from a population of cells sought to be transfected or infected by the viral vector. In other aspects, the selectable marker may be carried on a separate piece of DNA and used in a co-transfection procedure. Both the selectable marker and the reporter gene may be flanked by appropriate regulatory sequences to enable expression in a host cell. Useful selectable markers include, for example, antibiotic resistance genes, such as neo and the like.
Suitable reporter genes may include genes encoding luciferase, β -galactosidase, chloramphenicol acetyltransferase, secreted alkaline phosphatase, or green fluorescent protein.
Methods for introducing and expressing genes into cells are known in the art. The vector may be readily introduced into a host cell by any method known in the art, for example, mammalian, bacterial, yeast or insect cells. For example, the expression vector may be transferred into a host cell by physical, chemical or biological means.
Physical methods for introducing nucleic acids into host cells include calcium phosphate precipitation, lipofection, particle bombardment, microinjection, electroporation, and the like. Biological methods for introducing a nucleic acid of interest into a host cell include the use of DNA and RNA vectors. Chemical means of introducing nucleic acids into host cells include colloidal dispersion systems such as macromolecular complexes, nanocapsules, microspheres, beads; and lipid-based systems including oil-in-water emulsions, micelles, mixed micelles, and liposomes.
Biological methods for introducing nucleic acids into host cells include the use of viral vectors, particularly lentiviral vectors, which have become the most widely used method for inserting genes into mammalian, e.g., human, cells. Other viral vectors may be derived from retroviruses, poxviruses, herpes simplex virus I, adenoviruses, adeno-associated viruses, and the like. Many virus-based systems have been developed for gene transfer into mammalian cells. For example, retroviruses provide a convenient platform for gene delivery systems. The selected gene can be inserted into a vector and packaged into a retroviral particle using techniques known in the art. The recombinant virus can then be isolated and delivered to the subject cells in vivo or ex vivo. Many retroviral systems are known in the art. In some embodiments, an adenoviral vector is used. Many adenoviral vectors are known in the art.
Thus, in certain embodiments, the invention also provides a lentivirus for activating T cells, the virus comprising a lentiviral vector as described herein and a corresponding packaging gene, such as gag, pol, and vsvg.
Thus, in certain embodiments, the invention provides a genetically modified T cell comprising a nucleic acid sequence as described herein, or comprising a lentiviral vector as described herein, or infected with a lentivirus as described herein, or prepared by a method as described herein, or stably expressing a fusion protein as described herein.
The CAR-T cells of the invention can undergo robust in vivo T cell expansion and sustained at high levels in the blood and bone marrow for extended amounts of time, and form specific memory T cells. Without wishing to be bound by any particular theory, the CAR-T cells of the invention can differentiate into a central memory-like state in vivo upon encountering and subsequently depleting target cells expressing a surrogate antigen.
The invention also includes a class of cell therapies in which T cells are genetically modified to express a CAR described herein, and the CAR-T cells are injected into a recipient in need thereof. The injected cells are capable of killing tumor cells of the recipient. Unlike antibody therapy, CAR-T cells are able to replicate in vivo, resulting in long-term persistence that can lead to sustained tumor control.
The anti-tumor immune response elicited by the CAR-T cells can be an active or passive immune response. Additionally, the CAR-mediated immune response can be part of an adoptive immunotherapy step, in which the CAR-T cells induce an immune response specific for the antigen-binding portion in the CAR.
Thus, the diseases that can be treated with the CARs, their coding sequences, nucleic acid vectors, expression vectors, viruses, and CAR-T cells of the invention are preferably CD 30-mediated diseases.
In particular, herein, "CD 30-mediated diseases" include, inter alia, various types of brain, bladder, breast, cervical, colorectal, liver, kidney, lymphoma, leukemia, lung, melanoma, metastatic melanoma, mesothelioma, neuroblastoma, ovarian, prostate, pancreatic, renal, skin, thymoma, sarcoma, non-hodgkin's lymphoma, uterine cancer. In certain embodiments, the CD 30-mediated disease is non-hodgkin's lymphoma, hodgkin's lymphoma.
The CAR-modified T cells of the invention can be administered alone or as a pharmaceutical composition in combination with diluents and/or with other components such as relevant cytokines or cell populations. Briefly, a pharmaceutical composition of the invention may comprise CAR-T cells as described herein, in combination with one or more pharmaceutically or physiologically acceptable carriers, diluents, or excipients. Such compositions may include buffers such as neutral buffered saline, sulfate buffered saline, and the like; carbohydrates such as glucose, mannose, sucrose or dextran, mannitol; a protein; polypeptides or amino acids such as glycine; an antioxidant; chelating agents such as EDTA or glutathione; adjuvants (e.g., aluminum hydroxide); and a preservative.
The pharmaceutical compositions of the present invention may be administered in a manner suitable for the disease to be treated (or prevented). The amount and frequency of administration will be determined by such factors as the condition of the patient, and the type and severity of the patient's disease.
When referring to an "immunologically effective amount", "an anti-tumor effective amount", "a tumor-inhibiting effective amount", or a "therapeutic amount", the precise amount of the composition of the invention to be administered can be determined by a physician, taking into account the age, weight, tumor size, extent of infection or metastasis, and individual differences in the condition of the patient (subject). It can be generally pointed out that: pharmaceutical compositions comprising T cells described herein can be in the range of 104To 109Dosage of individual cells/kg body weight, preferably 105To 106Dosage of individual cells/kg body weight. The T cell composition may also be administered multiple times at these doses. Cells can be administered by using infusion techniques well known in immunotherapy (see, e.g., Rosenberg et al, New Eng.J.of Med.319:1676, 1988). Optimal dosages and treatment regimens for a particular patient can be readily determined by those skilled in the medical arts by monitoring the patient for signs of disease and adjusting the treatment accordingly.
Administration of the subject composition may be carried out in any convenient manner, including by spraying, injection, swallowing, infusion, implantation or transplantation. The compositions described herein can be administered to a patient subcutaneously, intradermally, intratumorally, intranodal, intraspinally, intramuscularly, by intravenous injection, or intraperitoneally. In one embodiment, the T cell composition of the invention is administered to a patient by intradermal or subcutaneous injection. In another embodiment, the T cell composition of the invention is preferably administered by intravenous injection. The composition of T cells can be injected directly into the tumor, lymph node or site of infection.
In some embodiments of the invention, the CAR-T cells of the invention or compositions thereof can be combined with other therapies known in the art. Such therapies include, but are not limited to, chemotherapy, radiation therapy, and immunosuppressive agents. For example, treatment may be combined with radiation or chemotherapeutic agents known in the art for the treatment of CD30 mediated diseases.
The present invention is described in further detail by referring to the following experimental examples. These examples are provided for illustrative purposes only and are not intended to be limiting unless otherwise specified. Accordingly, the present invention should in no way be construed as limited to the following examples, but rather should be construed to include any and all variations which become apparent in light of the teachings provided herein. The methods and reagents used in the examples are, unless otherwise indicated, conventional in the art.
Example 1 chimeric antigen receptor preparation
The invention provides a chimeric antigen receptor targeting humanized CD 30. The design sequentially comprises DAP12, T2A, humanized CD30 single-chain variable region and TREM1, and the structure of the design is shown in figure 1.
The pELNS-DAP12-T2A plasmid was stored by Nanjing Katsui medicine science, Inc., or was constructed according to the method disclosed in the literature (EnxiuWang et al, Generation of patent T-cell Immunology for Cancer Using DAP12-Based, Multichain, Chimeric Immunoreppers.2015, Cancer Immunology Research,3(7):815), the CD30 scFv-TREM1 gene synthesis was synthesized and provided by Biotech, Inc., of Biotech, Inc., the plasmid pELNS-DAP12-T2A was separately synthesized with the synthesized gene fragment by double digestion with SalI (from Takara), the digestion was performed as described, and the BamHI was ligated to obtain a lentiviral vector expressing a Chimeric antigen receptor:
5 mu.L of lentiviral vector was transformed into E.coli TOP10 competent cells (purchased from Nanjing Ande high Biotech Co., Ltd.), and after culturing at 37 ℃ for 16h, monoclonals were picked up, and after culturing at 37 ℃ for 12h, plasmids were extracted with a plasmid extraction kit (purchased from Takara Co., Ltd.), and the specific method is described in the specification.
Example 2 Lentiviral packaging
The slow virus is packaged by a calcium phosphate method, and the method comprises the following specific steps:
293T cells were passaged every other day, 5X 10 cells were seeded per T150 cell flask6And (4) cells. After 48 hours, the cell number should reach 20-25 million/vial. In the case of 1T 150 cell culture flask, the cells were gently washed twice with about 15ml of 1 XPBS, 3ml of 0.25% pancreatin-2.21 mM EDTA was added until the cells were exfoliated, 12ml of 10% (wt) FBS (from Gibico) DMEM medium (from corning) was added to the exfoliated cells, the cells were collected and transferred to a sterile centrifuge tube, 1000rpm was applied, the cell was centrifuged for 10 minutes, the supernatant was aspirated, and the pellet was resuspended in 10ml of 10% (wt) FBS DMEM medium. Cell count, 12X 10 from cell concentration6The required volume of each cell, cells and 25ml of 10% (wt) FBS DMEM medium were combined, placed in a T150 cell flask, and shaken gently to distribute the cells evenly to the bottom of the cell flask at 37 deg.C and cultured overnight in a 5% CO2 incubator.
Cells were observed to reach a cell density of approximately 80% -90% at which time transfection was initiated by gently aspirating the medium 30-60 minutes prior to transfection. Plasmid DNA and calcium chloride solution were mixed, and one T150 vial was used as an example, 28ug pRSV.rev (available from Invitrogen), 28ug pGAG-Pol (available from Invitrogen), 11ug pVSVG (available from Invitrogen), and 23ug recombinant lentivirus expression plasmid CD30 CAR were added to 1.5ml of calcium chloride solution and mixed well. Adding 1.5ml of BBS solution into a 15ml sterile centrifuge tube, uniformly mixing the DNA-calcium chloride solution with a 1ml gun head, dropwise adding the mixture into the BBS solution, rapidly mixing the mixture uniformly for 15-20 ℃, and incubating the mixture for 25-30 minutes at room temperature. The DNA-calcium chloride-BBS mixture (available from Shanghai Bintian Biotechnology Co., Ltd.) was added dropwise to the T150 bottle uniformly using a 5ml pipette. Culturing in a cell culture box containing 5% carbon dioxide at 37 deg.C for 6 hr. And changing the liquid after 6 h. The plate was gently shaken several times to suspend some calcium phosphate precipitate sufficiently, the culture solution containing calcium phosphate precipitate was aspirated, 20ml of fresh 5% (wt) FBS DMEM culture solution was added, and the culture was continued.
The 293T cell culture supernatant transfected the previous day was collected into a centrifuge tube, centrifuged at 1000rpm for 5 minutes, labeled, and stored in a 4 ℃ freezer. 20ml of 5% (wt) FBS DMEM medium previously preheated was added to the cell flask and the cell culture was continued overnight in the cell incubator at 37 ℃. The viral supernatant was collected a second time (48 h/day). The supernatants from both collections were pooled together and filtered through a 0.45 μm filter to remove cellular debris. Centrifuging at 12000-24000rpm for one night at 4 ℃, pouring all supernatant after centrifugation, adding fresh 5% (wt) of FBS DMEM culture medium for resuspension, performing virus subpackaging, and rapidly storing in a refrigerator at-80 ℃ for later use.
Example 3 viral infection of T cells
Collecting peripheral blood by using a blood collection tube containing an anticoagulant, naturally settling for about 30min at room temperature (18-25 ℃), collecting upper plasma, centrifuging the collected upper plasma for 10min at 5000r/min, adding the collected upper plasma to a lymphocyte separation solution (purchased from Tianjin Shangjing Biotechnology Limited liability company) according to a volume ratio of 1:1, carrying out gradient centrifugation for 3000r/min, centrifuging for 30min, and after centrifugation, layering a centrifugal tube from top to bottom: the first layer is a plasma layer; the second layer is a lymphocyte leucocyte layer; the third layer is a transparent separation liquid layer; the fourth layer of red blood cells. Sucking lymphocyte leucocyte membrane layer, washing with PBS for 2 times, centrifuging twice at 1500r/min for 10min, resuspending cells with PBS, adding 5% autologous plasma +300IU/ml recombinant human IL-2+ KBM581 complete culture medium to culture human peripheral blood mononuclear cells. Freshly prepared mononuclear cell PBMC were cultured in complete medium containing 5% autologous plasma +300IU/ml recombinant human IL-2+ KBM581, IL-2 from R & D Systems, KBM581 from Corning, CD3/CD28 Dynabeads immunomagnetic beads (from invitrogen) added on day 0 to activate T cells, lentiviral infection was performed the first 3 days, 0.25MOI corresponding lentiviral vector was added, uninfected T lymphocytes were used as a blank, after 48h the medium was changed to complete medium containing 5% autologous plasma +300IU/ml recombinant human IL-2+ KBM581, and culture was continued for 7-9 days.
Example 4 Effect of viral infection of CAR-T cells on cell proliferation
After lentivirus infection of T cells, the T cells were counted every 1-2 days in complete medium containing a volume fraction of 5% autologous plasma +300IU/ml recombinant human IL-2+ KBM 581. T lymphocyte growth was then observed, and the results are shown in FIG. 3. The results show that the cells can still form typical proliferation clone masses after being infected by the CAR-expressing virus, and the proliferation curves of the cells are drawn to show that the proliferation capacity of infected CD30 CAR-T cells is slightly weaker than that of T cells (NTD in figure 3) which are not infected by the virus.
Example 5 detection of cytokine secretion by Virus-infected CAR-T cells
(1) Cytokine detection was performed by the method of Elisa using a kit of R & D.
(2) And (3) diluting the standard: preparing 7 centrifuge tubes of 1ml, numbering in sequence, firstly adding 500 mu L of standard substance diluent into each centrifuge tube, then adding 500 mu L of original concentration standard substance into 1 numbered centrifuge tube, fully and uniformly mixing, then adding 500 mu L of standard substance into a second centrifuge tube in the centrifuge tube, and fully and uniformly mixing; then taking 500 mu L of the centrifugal tube, adding the centrifugal tube into a third centrifugal tube, and fully and uniformly mixing; then taking 500 mu L of the centrifugal tube, adding the centrifugal tube into a fourth centrifugal tube, and fully and uniformly mixing; then taking 500 mu L of the centrifugal tube, adding the centrifugal tube into a fifth centrifugal tube, and fully and uniformly mixing; then taking 500 mu L of the centrifugal tube, adding the centrifugal tube into a sixth centrifugal tube, and fully and uniformly mixing; then, 500. mu.L of the suspension was added to a seventh centrifuge tube and mixed well.
(3) And standard substance holes are formed in the enzyme-labeled coating plate, and 100 mu L of standard substances with different concentrations are sequentially added, wherein each concentration is 2-3 parallel holes.
(4) Sample adding: respectively arranging blank holes (the blank control hole is replaced by water, the enzyme labeling reagent and the biotin-labeled antibody are operated as before) and sample holes to be detected, adding 100 mu L of sample in the sample holes to be detected on the enzyme labeling coated plate, adding the sample to the bottom of the plate hole of the enzyme labeling plate, keeping the hole wall untouched as far as possible, gently shaking and uniformly mixing
(5) And (3) incubation: standing at room temperature for incubation for 2h
(6) Washing: discarding liquid, spin-drying, adding 200 μ L of washing solution into each well, standing for 30s, discarding, repeating for 3 times, and patting to dry
(7) Adding an antibody: adding 100 mu L of detection antibody on the enzyme-labeled coated plate
(8) And (3) incubation: same operation (5)
(9) Washing: same operation (6)
(10) Marking: 100 μ L of horseradish peroxidase-labeled streptavidin was added to each well
(11) And (3) incubation: incubating at room temperature in dark for 20min
(12) Washing: same operation (6)
(13) Color development: adding 100 μ L of color development liquid into each well, shaking gently, mixing, incubating at room temperature in dark for 20min
(14) And (4) terminating: stop solution (50. mu.L) was added to each well to stop the reaction
(15) And (3) determination: the blank value is used for zero calibration, the absorbance (OD value) of each hole is measured in sequence at the wavelength of 450nm, and the measurement is carried out within 15min after the stop solution is added.
Selecting target cells with different antigen expression levels to be cultured with CD30 CAR-T, detecting whether the CD30 CAR-T responds to antigen stimulation to secrete IFN-gamma level, selecting 293T-CD30 (highly expressed CD 30) and 293T (negative CD 30) as target cells, and displaying that the CD30 CAR-T specifically secretes IFN-gamma when stimulated by CD30 antigen, and reflecting that the CD30 CAR responds to the target cells with different antigen expression levels. CD30 CAR-T secreted significantly IFN- γ when co-cultured with CD30 high expressing target cells 293T-CD30 (fig. 4), indicating that CD30 CAR-T had a response effect on antigen positive tumor cells.
Example 6 evaluation of the killing Effect of virally infected CAR-T cells in vitro
(1) Respectively culturing 293T-CD30 cells (CD30 high expression cell strain), 293T (CD30 negative cell strain) and CD30 CAR-T cells serving as effector cells.
(2) Collecting target cells and effector cells, centrifuging at 1500rpm/min for 5min, discarding supernatant
(3) Resuspension of target and effector cells in 10% FBS +1640 complete Medium
(4) Using a real-time cell analysis System (RTCA), 50. mu.L 1640 medium was added to the E-Plate16 in air
(5) Determining normal contact of selected holes using RTCA baseline detection
(6) Setting the effective target ratio to be 0:1, 1:1, 5:1, 10:1
(7) E-Plate16 was removed and 100. mu.L of the well-mixed target cell suspension was added to each well in an effective target ratio so that the number of each cell was 104cells/100μL。
(8) E-Plate16 was placed in an incubator at 37 ℃ under 5% CO2 overnight
(9) The next day, E-Plate16 was removed, 50. mu.L of the corresponding effector cells were added, and the killing rate 8h after the addition of the effector cells was calculated.
(10)
Figure BDA0002383127790000121
The results of the detection are shown in FIG. 5. CD30 CAR-T showed significant killing effect on CD30 antigen positive tumor cells. The results of fig. 4 and 5 show that the results of in vitro killing experiments show that the CAR-T cells targeting CD30 have significant anti-tumor activity, and the CAR design is beneficial to clinical application.
Finally, it is noted that the above-mentioned preferred embodiments illustrate rather than limit the invention, and that, although the invention has been described in detail with reference to the above-mentioned preferred embodiments, it will be understood by those skilled in the art that various changes in form and detail may be made therein without departing from the scope of the invention as defined by the appended claims.
Sequence listing
<110> Nanjing Aide immunotherapy research institute Co., Ltd
<120> chimeric antigen receptor targeting humanized CD30 and uses thereof
<130>2019
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agacggaggc ctggacacga tctggaatgg attggataca ttaatcctag cagtggatgt 660
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Lys Val Glu Gly Gly Gly Glu Gly Arg Gly Ser Leu Leu Thr Cys Gly
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465

Claims (9)

1. A nucleic acid sequence selected from the group consisting of: contains the coding sequence of human DAP12, T2A, anti-CD 30 single-chain antibody and human TREM1 transmembrane and intracellular region connected in sequence.
2. The nucleic acid sequence as claimed in claim 1, wherein the nucleic acid sequence further comprises a nucleic acid sequence of a signal peptide before the coding sequence of the anti-CD 30 single-chain antibody, preferably the nucleic acid sequence of the signal peptide is as shown in SEQ ID NO 1, nucleic acid 412-474; and/or the nucleic acid sequence of the anti-CD 30 antibody is shown as the 481-1236 polynucleic acid of SEQ ID NO. 1; and/or the nucleic acid sequence of the human DAP12 is shown as the 1 st-339 st polynucleic acid of SEQ ID NO 1; and/or the nucleic acid sequence of the T2A is shown as the 355-405 th nucleic acid of SEQ ID NO. 1; and/or the nucleic acid sequence of the transmembrane and intracellular region of the human TREM1 is shown as the 1273-1410 nucleic acid of SEQ ID NO: 1.
3. A fusion protein selected from the group consisting of: a fusion protein containing sequentially connected human DAP12, T2A, anti-CD 30 single-chain antibody, human TREM1 transmembrane and intracellular regions; and a derivative fusion protein in which one or more amino acids are substituted, deleted or added in the defined amino acid sequence and which retains the activity of activated T cells; preferably, the anti-humanized CD30 monoclonal antibody is huggn-35.
4. The fusion protein of claim 3, wherein the fusion protein has one or more of the following characteristics: the fusion protein also comprises a signal peptide at the N end of the anti-CD 30 antibody, preferably, the amino acid sequence of the signal peptide is shown as the amino acid at the 138 th-158 th position of SEQ ID NO. 2; the amino acid sequence of the anti-CD 30 single-chain antibody is shown as the amino acid position 161-412 of SEQ ID NO. 2; the amino acid sequence of the human DAP12 is shown as amino acids 1-113 of SEQ ID NO. 2; the amino acid sequence of the T2A is shown as the 119 th and 135 th amino acids of SEQ ID NO 2; the amino acid sequence of the transmembrane and intracellular region of the human TREM1 is shown as amino acids 425-469 of SEQ ID NO 2.
5. A nucleic acid vector comprising the nucleic acid sequence of any one of claims 1-2; preferably, the nucleic acid vector is a lentiviral vector comprising the nucleic acid sequence of any one of claims 1-2.
6. A lentivirus comprising the nucleic acid vector of claim 5, preferably said lentivirus vector.
7. A genetically modified T-cell or a pharmaceutical composition comprising a genetically modified T-cell, wherein the cell comprises the nucleic acid sequence of any one of claims 1-2, or comprises the nucleic acid vector of claim 5, or is infected with the lentivirus of claim 6, or stably expresses the fusion protein of claim 4.
8. Use of the nucleic acid sequence of any one of claims 1-2, the fusion protein of any one of claims 3-4, the nucleic acid vector of claim 5, or the lentivirus of claim 7 for the preparation of activated T cells.
9. Use of the nucleic acid sequence of any one of claims 1-2, the fusion protein of any one of claims 3-4, the nucleic acid vector of claim 5, the lentivirus of claim 6, or the genetically modified T cell of claim 7, or a pharmaceutical composition thereof, in the manufacture of a medicament for treating a CD 30-mediated disease; preferably, the CD 30-mediated disease is brain cancer, bladder cancer, breast cancer, cervical cancer, colorectal cancer, liver cancer, kidney cancer, lymphoma, leukemia, lung cancer, melanoma, metastatic melanoma, mesothelioma, neuroblastoma, ovarian cancer, prostate cancer, pancreatic cancer, kidney cancer, skin cancer, thymoma, sarcoma, non-hodgkin lymphoma, uterine cancer, preferably non-hodgkin lymphoma, hodgkin lymphoma.
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Application publication date: 20200609