TECHNICAL FIELD
The present disclosure relates to the field of biotechnology, in particular to a method for performing gene editing on a target site in a cell.
CRISPR/Cas9 system is an acquired immune mechanism derived from archaea and bacteria that protects against the invasion of exogenous DNA fragments such as plasmids and phages. The system mainly functions by CRISPR sequences and loci encoding Cas proteins. Cas9 nucleases, belong to the type II family, are currently most commonly used, in which only a single effector protein can function. When exogenous DNA invades bacteria, the type II CRISPR system first integrates the invading DNA between CRISPR repeat sequences. Subsequently, CRISPR RNAs (crRNAs) containing invading DNA sequences are transcribed and processed. Thereafter, trans-activating crRNA (tracrRNA) binds to crRNA and eventually forms a complex with the Cas9 protein. Finally, the Cas9 protein acts as an endonuclease to trigger DNA double-strand breaks through its HNH and RuvC-like domains. Double-strand DNA breaks trigger damage repair mechanisms, and when homologous templates are present, cells can undergo precise homologous recombination repair, which allows the insertion or replacement of exogenous sequences. So far, CRISPR/Cas9 technology has been successfully applied in many fields and shows broad prospects. However, there are still many difficulties in precise gene therapy using homologous recombination, and one of the main limiting factors is that the efficiency of homologous recombination is very low. Although a number of studies have reported a variety of methods to increase homologous recombination efficiency, increasing evidence shows that these methods are not applicable for all types of cells and the effects are not consistent. Therefore, finding personalized approaches to effectively improve homologous recombination in specific cells is particularly important for cell type-based cell therapy.
Chimeric Antigen Receptor T-Cell (CAR-T) is a novel adoptive immunotherapy emerging in recent years. It genetically modifies patients' T cells in vitro and reinfuses them into patients after expansion, achieving targeted killing of tumors. At present, three CAR-T products have been approved by the US Food and Drug Administration for the clinical treatment of hematological malignancies, demonstrating the great success of CAR-T technology. However, as emerging technologies, CAR-T technology still faces many challenges in various aspects and has huge room for improvement. First, the most commonly used method nowadays is to introduce exogenous sequences using viral systems. However, the use of virus systems has the problems of high preparation cost and potential safety risks with random insertion. Secondly, traditional technologies, including viral preparation are unable to achieve precise insertion of exogenous sequences into the genome, which can cause poor cell homogeneity and affect the therapeutic effect, and fail to engineer T cells diversely. In addition, CAR-T therapy is currently a personalized treatment, which has problems such as high production cost, long preparation time, limited effects and other problems. Therefore, it is important to achieve site-specific integration of artificial modified elements such as CAR in T cells using technologies such as CRISPR/Cas9 to promote the development of existing T cell therapy. On the one hand, it can avoid the uncertainty caused by random insertion of exogenous sequences and improve the homogeneity and robustness of cell products. On the other hand, it can achieve versatile transformation of T cells, which can not only construct universal CAR-T cells in one step, construct enhanced cell products by regulating endogenous genes, but also achieve the dynamic expression of artificial elements, which is of great help to expand the application of current technologies. However, due to the property of T cells, the efficiency of site-directed integration of exogenous sequences by homologous recombination is very low. Therefore, there is an urgent need to develop a method to improve the efficiency of homologous recombination in T cells in this field.
One of the purposes of the present invention is to provide a novel method to improve the efficiency of homologous recombination of an exogenous sequence in a cell (especially T cell).
The invention provides a method of gene editing for genes AAVS1, PD1, TRAC and B2M, respectively.
The first aspect of the present invention provides a method for performing gene editing on a target site of a cellular genome comprising:
In another preferred embodiment, the gene editing comprises gene knock-out and gene-targeted integration.
In another preferred embodiment, when the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 1-6, the gene editing is gene-targeted integration.
In another preferred embodiment, when the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 7-9, the gene editing is gene knock-out.
In another preferred embodiment, the enzyme for gene editing is selected from the group consisting of CRISPR related protein (Cas) polypeptide, TALEN enzyme, ZFN enzyme, or combinations thereof.
In another preferred embodiment, the enzyme for gene editing is derived from a microorganism; preferably derived from a bacterium.
In another preferred embodiment, the source of the enzyme for gene editing is selected from the group consisting of Streptococcus pyogenes, Staphylococcus aureus, Streptococcus canis or combinations thereof.
In another preferred embodiment, the enzyme for gene editing comprises a wild-type or mutated enzyme for gene editing.
In another preferred embodiment, the enzyme for gene editing is selected from the group consisting of Cas9, Cas12, Cas13, Cms1, MAD7, Cas3, Cas8a, Cas8b, Cas10d, Cse1, Csy1, Csn2, Cas4, Cas10, Csm2, Cmr5, Fok1, Cpf1 or combinations thereof.
In another preferred embodiment, the gRNA comprises crRNA, tracrRNA, sgRNA.
In another preferred embodiment, the gRNA targets and binds to the target site of the genome.
In another preferred embodiment, the gRNA comprises a gRNA without or with a modification.
In another preferred embodiment, the gRNA with a modification comprises a chemical modification on a base.
In another preferred embodiment, the chemical modification comprises methylation modification, methoxy modification, fluorination modification or sulfur modification.
In another preferred embodiment, the gene editing comprises in vivo gene editing, in vitro gene editing.
In another preferred embodiment, the gene editing comprises CRISPR based gene editing.
In another preferred embodiment, the target site is selected from the group consisting of AAVS1, PD1, TRAC, B2M or combinations thereof.
In another preferred embodiment, the target sequence targeted by the gRNA for AAVS1 comprises the sequence shown in SEQ ID NO: 3.
In another preferred embodiment, the target sequence targeted by the gRNA for PD1 comprises the sequence shown in SEQ ID NO: 1 and/or SEQ ID NO: 2.
In another preferred embodiment, the target sequence targeted by the gRNA for TRAC comprises the sequence shown in SEQ ID NO: 4 and/or SEQ ID NO: 5.
In another preferred embodiment, the target sequence targeted by the gRNA for B2M comprises the sequence shown in SEQ ID NO: 6.
In another preferred embodiment, the gene editing comprises a site-directed knock-in of a DNA donor.
In another preferred embodiment, the DNA donor is double-stranded DNA.
In another preferred embodiment, the DNA donor comprises a first homology arm and a second homology arm, wherein the first homology arm and the second homology arm are capable of initiating a cell-mediated homologous recombination of the DNA donor at the target site of the cellular genome, and the sequence lengths of each of the first homology arm and the second homology arm are independently 200-2000 bp, preferably 400-1000 bp, more preferably 700-900 bp.
In another preferred embodiment, the first homology arm is homologous to the sequence upstream-side (or left-side) of the cleavage site of the target site in the genome, while the second homology arm is homologous to the sequence downstream-side (or right-side) of the cleavage site of the target site in the genome.
In another preferred embodiment, the DNA donor comprises a target gene.
In another preferred embodiment, the target gene comprises a coding sequence of a chimeric antigen receptor or a TCR.
In another preferred embodiment, the sequence length of the DNA donor is 50 bp-5000 bp, preferably 80 bp-4000 bp.
In another preferred embodiment, the sequence length of the target gene is 50 bp-3000 bp, preferably 1000 bp-2000 bp.
In another preferred embodiment, the sequence length of the coding sequence of the chimeric antigen receptor or TCR is 50 bp-3000 bp, preferably 1000 bp-2000 bp.
In another preferred embodiment, the ratio (D1/D2) of the sequence length of the first homology arm (D1) to the sequence length of the second homology arm (D2) is (0.8-1.2):(0.5-1.5), preferably (0.9-1.1):(0.7-1.3), more preferably, 1:1.
In another preferred embodiment, the chimeric antigen receptor contains an antigen binding domain targeting a tumor cell marker.
In another preferred embodiment, the chimeric antigen receptor comprises an antigen binding domain targeting a tumor cell marker, an optional hinge region, a transmembrane domain and an intracellular signal transduction binding domain.
In another preferred embodiment, the tumor cell marker is selected from the group consisting of folate receptor α, 5T4, αvβ6 integrin, BCMA, B7-H3, B7-H6, CAIX, CD16, CD19, CD20, CD22, CD30, CD33, CD44, CD44v6, CD44v7/8, CD70, CD79a, CD79b, CD123, CD138, CD171, CEA, CSPG4, EGFR, EGFR family including ErbB2 (HER2), EGFRvIII, EGP2, EGP40, EPCAM, EphA2, EpCAM, FAP, fetal AchR, FRα, GD2, GD3, phosphatidylinositol proteoglycan-3 (GPC3), HLA-A1+MAGE1, HLA-A2+MAGE1, HLA-A3+MAGE1, HLA-A1+NY-ESO-1, HLA-A2+NY-ESO-1, HLA-A3+NY-ESO-1, IL-11Rα, IL-13Rα2, Lambda, Lewis-Y, Kappa, mesothelin, Muc1, Muc16, NCAM, NKG2D ligand, NY-ESO-1, PRAME, PSCA, PSMA, ROR1, SSX, survivin, TAG72, TEM, VEGFR2, WT-1, or combinations thereof.
In another preferred embodiment, the hinge region is a hinge region of a protein selected from the group consisting of CD8, Ig (immunoglobulin) hinge, CD28, or combinations thereof.
In another preferred embodiment, the transmembrane domain is a transmembrane domain of a protein selected from the group consisting of CD8α, CD8β, CD28, CD33, CD37, CD5, CD16, ICOS, CD9, CD22, CD134, CD137, CD154, CD19, CD45, CD4, CD3ε, CD3γ, CD3ζ, or combinations thereof.
In another preferred embodiment, the intracellular signal transduction binding domain comprises a costimulatory signaling molecule and/or a primary signal transduction domain.
In another preferred embodiment, the costimulatory signaling molecule is selected from the group consisting of OX40, CD28, CD30, CD40, CD70, CD134, 4-1BB (CD137), LIGHT, DAP10, CDS, ICAM-1, CD278 (ICOS), TLR1, TLR2, TLR3, TLR4, TLR5, TLR6, TLR7, TLR8, TLR9, TLR10, CARD11, CD2, CD7, CD27, CD54 (ICAM), CD83, LAT, NKD2C, SLP76, TRIM, ZAP70, or combinations thereof.
In another preferred embodiment, the primary signal transduction domain is selected from the group consisting of FcRγ, FcRβ, CD3γ, CD3δ, CD3ε, CD3ζ, CD22, CD79a, CD79b, CD66d, or combinations thereof.
In another preferred embodiment, the sequence of the DNA donor is shown in any one of SEQ ID NO: 12-38.
In another preferred embodiment, the cell comprises a primary cell and a subcultured cell.
In another preferred embodiment, the cell comprises a T cell.
In another preferred embodiment, the cell comprises a CD3+ T cell, a CD4+ helper T cell, a CD4+ regulatory T cell, a CD8+ T cell and a memory T cell.
In another preferred embodiment, the vector comprises a viral vector.
In another preferred embodiment, the viral vector is selected from the group consisting of an adeno-associated viral vector, a lentiviral vector, or combinations thereof.
In another preferred embodiment, the method for introducing comprises electrotransport, vector transformation, transfection, heat shock, electroporation, transduction, gene gun, microinjection, liposome transfection and lentivirus infection.
In another preferred embodiment, the method is an in vitro method.
In another preferred embodiment, the method is non-diagnostic or non-therapeutic.
The second aspect of the present invention provides a gRNA for gene editing on a target site of a cellular genome, wherein the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 1-9.
In another preferred embodiment, the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 1-6.
In another preferred embodiment, the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 7-9.
In another preferred embodiment, the gRNA comprises a gRNA without or with a modification.
In another preferred embodiment, the gRNA with a modification comprises a chemical modification on a base.
In another preferred embodiment, the chemical modification comprises methylation modification, methoxy modification, fluorination modification or sulfur modification.
The third aspect of the present invention provides a reaction system for gene editing on a target site of a cellular genome comprising:
In another preferred embodiment, the gene editing comprises gene knock-out and gene-targeted integration.
In another preferred embodiment, when the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 1-6, the gene editing is gene-targeted integration.
In another preferred embodiment, when the targeting sequence targeted by the gRNA comprises one or more of the sequences shown in SEQ ID NO: 7-9, the gene editing is gene knock-out.
In another preferred embodiment, the target site is selected from the group consisting of AAVS1, PD1, TRAC, B2M or combinations thereof.
In another preferred embodiment, the target sequence targeted by the gRNA for AAVS1 comprises the sequence shown in SEQ ID NO: 3.
In another preferred embodiment, the target sequence targeted by the gRNA for PD1 comprises the sequence shown in SEQ ID NO: 1 and/or SEQ ID NO: 2.
In another preferred embodiment, the target sequence targeted by the gRNA for TRAC comprises the sequence shown in SEQ ID NO: 4 and/or SEQ ID NO: 5.
In another preferred embodiment, the target sequence targeted by the gRNA for B2M comprises the sequence shown in SEQ ID NO: 6.
In another preferred embodiment, the DNA donor comprises a first homology arm and a second homology arm, wherein the first homology arm and the second homology arm are capable of initiating an immune cell-mediated homologous recombination of the DNA donor at the target site of the genome of the immune cell, and the sequence lengths of each of the first homology arm and the second homology arm are independently 200-2000 bp, preferably 400-1000 bp, more preferably 700-900 bp.
In another preferred embodiment, the DNA donor comprises a target gene.
In another preferred embodiment, the target gene comprises a coding sequence of a chimeric antigen receptor or a TCR.
In another preferred embodiment, the chimeric antigen receptor contains an antigen binding domain targeting a tumor cell marker.
In another preferred embodiment, the chimeric antigen receptor comprises an antigen binding domain targeting a tumor cell marker, an optional hinge region, a transmembrane domain and an intracellular signal transduction binding domain.
In another preferred embodiment, the tumor cell marker is selected from the group consisting of folate receptor α, 5T4, αvβ6 integrin, BCMA, B7-H3, B7-H6, CAIX, CD16, CD19, CD20, CD22, CD30, CD33, CD44, CD44v6, CD44v7/8, CD70, CD79a, CD79b, CD123, CD138, CD171, CEA, CSPG4, EGFR, EGFR family including ErbB2 (HER2), EGFRvIII, EGP2, EGP40, EPCAM, EphA2, EpCAM, FAP, fetal AchR, FRα, GD2, GD3, phosphatidylinositol proteoglycan-3 (GPC3), HLA-A1+MAGE1, HLA-A2+MAGE1, HLA-A3+MAGE1, HLA-A1+NY-ESO-1, HLA-A2+NY-ESO-1, HLA-A3+NY-ESO-1, IL-11Rα, IL-13Rα2, Lambda, Lewis-Y, Kappa, mesothelin, Muc1, Muc16, NCAM, NKG2D ligand, NY-ESO-1, PRAME, PSCA, PSMA, ROR1, SSX, survivin, TAG72, TEM, VEGFR2, WT-1, or combinations thereof.
In another preferred embodiment, the hinge region is a hinge region of a protein selected from the group consisting of CD8, Ig (immunoglobulin) hinge, CD28, or combinations thereof.
In another preferred embodiment, the transmembrane domain is a transmembrane domain of a protein selected from the group consisting of CD8α, CD8β, CD28, CD33, CD37, CD5, CD16, ICOS, CD9, CD22, CD134, CD137, CD154, CD19, CD45, CD4, CD3ε, CD3γ, CD3ζ, or combinations thereof.
In another preferred embodiment, the intracellular signal transduction binding domain comprises a costimulatory signaling molecule and/or a primary signal transduction domain.
In another preferred embodiment, the costimulatory signaling molecule is selected from the group consisting of OX40, CD28, CD30, CD40, CD70, CD134, 4-1BB (CD137), LIGHT, DAP10, CDS, ICAM-1, CD278 (ICOS), TLR1, TLR2, TLR3, TLR4, TLR5, TLR6, TLR7, TLR8, TLR9, TLR10, CARD11, CD2, CD7, CD27, CD54 (ICAM), CD83, LAT, NKD2C, SLP76, TRIM, ZAP70, or combinations thereof.
In another preferred embodiment, the primary signal transduction domain is selected from the group consisting of FcRγ, FcRβ, CD3γ, CD3δ, CD3ε, CD3ζ, CD22, CD79a, CD79b, CD66d, or combinations thereof.
In another preferred embodiment, the cell comprises a primary cell and a subcultured cell.
In another preferred embodiment, the cell comprises a T cell.
In another preferred embodiment, the cell comprises a CD3+ T cell, a CD4+ helper T cell, a CD4+ regulatory T cell, a CD8+ T cell and a memory T cells.
In another preferred embodiment, the first homology arm is homologous to the sequence upstream-side (or left-side) of the cleavage site of the target site in the genome, while the second homology arm is homologous to the sequence downstream-side (or right-side) of the cleavage site of the target site in the genome.
In another preferred embodiment, the sequence length of the DNA donor is 50 bp-5000 bp, preferably 80 bp-4000 bp.
In another preferred embodiment, the sequence length of the target gene is 50 bp-3000 bp, preferably 1000 bp-2000 bp.
In another preferred embodiment, the sequence length of the coding sequence of the chimeric antigen receptor or TCR is 50 bp-3000 bp, preferably 1000 bp-2000 bp.
In another preferred embodiment, the sequence of the DNA donor is shown in any one of SEQ ID NO: 12-38.
In another preferred embodiment, the vector comprises a viral vector.
In another preferred embodiment, the viral vector is selected from the group consisting of an adeno-associated viral vector, a lentiviral vector, or combinations thereof.
The fourth aspect of the present invention provides a kit for gene editing comprising:
In another preferred embodiment, the first container, the second container and the third container are the same container or different containers.
The fifth aspect of the present invention provides a gene-edited cell prepared by the method of the first aspect of the present invention.
The sixth aspect of the present invention provides a use of the cell of the fifth aspect of the present invention in the preparation of a product for tumor immunotherapy or cancer immunotherapy.
Those of skill in the art should be understood that, within the scope of the present invention, each of the above technical features and the technical features specifically described in the following (such as the examples) in the present invention can be combined with each other to form a novel or preferred technical solution. The details would not be described one by one herein due to the limitation of space.
In the figures of this application, “Untreated T” refers to untreated T cells, “Control” refers to T cells electroporated only with homologous templates and Cas9, “LV-19bbz” refers to CD19-CART cells prepared with lentivirus, “AAVS1-19bbz” refers to non-viral AAVS1 site-directed integrated CD19-CART cells, and “PD1-19bz” refers to non-viral PD1 site-directed integrated CD19-CART cells.
After extensive and intensive research, and through a large number of screening, the inventors accidentally screened gRNAs for highly efficient gene editing of target sites (such as: AAVS1, PD1, TRAC, B2M) for the first time. In addition, by comparing the first homology arm and the second homology arm of different lengths, the inventors further accidentally determined the conditions for highly efficient integration of the exogenous nucleic acid into the genome of T cells (such as highly efficient integration using the first homology arm and the second homology arm with specific lengths at genomic target sites). The present invention is completed on this basis.
CRISPR/Cas9 is an adaptive immune defense formed by bacteria and archaea during long-term evolution and can be used to fight invading viruses and exogenous DNA. The CRISPR/Cas9 system provides immunity by integrating fragments of invading phage and plasmid DNA into CRISPR and using corresponding CRISPR RNAs (e.g., gRNAs) to guide the degradation of homologous sequences.
The working principle of this system is that crRNA (CRISPR-derived RNA) binds to tracrRNA (trans-activating RNA) through base pairing to form a tracrRNA/crRNA complex, which guides the nuclease Cas9 protein to cleave double-stranded DNA at the target site with the sequence paired with crRNA. While these two RNAs can be engineered to form gRNAs (single-guide RNAs) with guiding function by artificial design, they are sufficient to guide the site-directed cleavage of DNA by Cas9.
As an RNA-directed dsDNA-binding protein, Cas9 effector nuclease is the first known unifying factor and is able to co-localize RNA, DNA, and protein. Fusion of the protein to nuclease-free Cas9 (Cas9 nuclease-null) and expression of the appropriate gRNA can target any dsDNA sequence, while the end of the gRNA can be attached to the target DNA without affecting Cas9 binding. Therefore, Cas9 can bring any fusion protein and RNA at any dsDNA sequence. This technology is called the CRISPR/Cas9 gene editing system.
In the targeted integration strategy of the present invention, a linearized donor (i.e., DNA donor or exogenous nucleic acid) containing a homology arm with a specific length is provided, which is a transgenic donor template containing a homology arm with a certain length (e.g., 700-900 bp) obtained by PCR amplification or precise digestion; DNA donor or exogenous nucleic acid is electroporated into cells along with Cas9 mRNA and guide RNA. The targeted integration strategy provided by the present invention has higher integration efficiency than the existing gene targeting strategy.
In the present invention, a linearized dsDNA donor (i.e., DNA donor or exogenous nucleic acid) consisting of a transgene fragment and 700-900 bp homology arms on either of the two sides is a key factor for achieving highly efficient targeted integration by CRISPR-mediated genome editing. The targeted integration technique of the present invention has the highest recombination efficiency compared to MMEJ (microhomology arm-mediated end-joining) or HITI (homology-independent targeted integration)-mediated methods.
The present invention provides a method for gene editing at a target site in a cellular genome, comprising:
The methods of the present invention enables highly efficient gene knock-out or gene-targeted integration at target sites (such as AAVS1, PD1, TRAC, B2M, etc.).
The present invention provides a reaction system for gene editing at a target site in a cellular genome comprising:
In a preferred embodiment, the DNA donor comprises a first homology arm and a second homology arm, wherein the first homology arm and the second homology arm are capable of initiating a homologous recombination of the DNA donor mediated by an immune cell at the target site in the immune cellular genome, and the sequence lengths of the first homology arm and the second homology arm are 200-2000 bp independently, preferably 400-1000 bp, more preferably 700-900 bp.
In the present invention, the sequence length of the DNA donor to be integrated can be 50 bp-5000 bp. The length of the target gene (or called target gene) in the DNA donor of the present invention may be 50 bp-3000 bp.
In the present invention, there is no special restriction on target sites, and one preferred target site includes AAVS1, PD1, TRAC, B2M.
In a preferred embodiment of the present invention, the ratio (D1/D2) of the sequence length of the first homology arm (D1) to the sequence length of the second homology arm (D2) is (0.8-1.2):(0.5-1.5), preferably (0.9-1.1):(0.7-1.3), more preferably 1:1.
In this reaction system, the sequence lengths of two homology arms are not required to be completely identical, and a certain length difference is allowed between them.
The main advantages of the present invention include:
The present invention is further elaborated in combination with specific embodiments. It should be understood that these embodiments are solely intended to describe the present invention and not to limit the scope of the present invention. Experimental methods that do not specify specific conditions in the following embodiments are generally performed according to conventional conditions such as those described in Sambrook et al., Molecular Cloning: Laboratory Manual (New York: Cold Spring Harbor Laboratory Press, 1989), or according to conditions described in the Microbiology: Laboratory Manual (James Cappuccino and Natalie Sherman, Pearson Education Press), or as suggested by the manufacturer. Human donor cells used in the experiments in the present invention were obtained from Shanghai SAILY Biological Technology Co., Ltd.
Materials and reagents used in the embodiments are commercially available unless otherwise specified.
Electroporation of T cells is a technical method to achieve gene editing of T cells, and the procedure is based on Lonza P3 Primary Cell 4D-Nucleofector® X kit.
Instruments and Materials:
Specific Operation Steps:
Applicable to 100 μL electroporation cuvette:
The CD19-CART sequence includes the extracellular domain targeting CD19, the transmembrane region of CD8α, and the intracellular signaling domains from CD3ζ and CD137.
The Celltiter One Solution Cell Proliferation Assay kit from Promega was used to detect the number of viable cells according to the instructions.
For example, non-viral site-directed integrated CD19-CART cells (including T cells with CAR integrated at AAVS1 safe harbor, T cells with CD19-CAR integrated at PD1 immune checkpoint locus, T cells with CD19-CAR integrated at TRAC locus, and T cells with CD19-CAR integrated at B2M locus) can be constructed in one step using the method of the invention combined with CRISPR/Cas9 technology.
1. Target sequence information
2. sgRNA was synthesized by the company and dissolved in TE buffer, and diluted to a final concentration of 10 μg/μL.
3. Preparation of non-viral site-directed integrated CD19-CART
Instruments and Materials:
Specific Operation Steps:
Applicable to 100 μL electroporation cuvette:
4. Evaluation of AAVS1 site-directed integrated CD19-CART cells
5. Evaluation of PD1 site-directed integrated CD19-CART cells
(2) The PD1 site-directed integrated CD19-CART cells constructed using the present invention have a stronger ability of cell expansion than CD19-CART cells prepared by lentivirus (
(3) Similar to CD19-CART cells prepared by lentivirus, the expression of activation surface markers was upregulated in PD1 site-directed integrated CD19-CART cells in response to tumor cells, with a more pronounced increase in CD137 expression (
(4) Similar to CD19-CART cells prepared by lentivirus, PD1 site-directed integrated CD19-CART cells could secrete cytokines in response to tumor cells, with a more pronounced increase in IFN-γ secretion (
(5) Compared with CD19-CART cells prepared by lentivirus, PD1 site-directed integrated CD19-CART cells constructed by this invention had stronger anti-tumor ability in vitro and in vivo (
In addition, it should be mentioned that this application uses linear double-stranded DNA (DNA donor) as an example to perform experiments as shown below.
Among them, the plasmid sequence is described as follows:
The sequence of DNA donor is identical to the “PD1 site 1 with site-directed integration of the mTurquoise2 sequence with 800 bp homology arms (HDR)” in the linear double-stranded DNA sequence, i.e. as shown in SEQ ID NO: 12.
The sequence of DNA donor is identical to the “PD1 site 2 with site-directed integration of the mTurquoise2 sequence with 800 bp homology arms (HDR)” in the linear double-stranded DNA sequence, i.e. as shown in SEQ ID NO: 13.
Linear double stranded DNA (DNA donor) is shown in any one of SEQ ID NO: 12-38.
Among them, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 12, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at PD1 site 2 is shown in SEQ ID NO: 13, the mTurquoise2 sequence with 200 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 14, the mTurquoise2 sequence with 400 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 15, the mTurquoise2 sequence with 1600 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 16, the mTurquoise2 sequence with 200 bp homology arms (HDR) site-directed integrated at PD1 site 2 is shown in SEQ ID NO:17, the mTurquoise2 sequence with 400 bp homology arms (HDR) site-directed integrated at PD1 site 2 is shown in SEQ ID NO:18, the mTurquoise2 sequence with 1600 bp homology arms (HDR) site-directed integrated at PD1 site 2 is shown in SEQ ID NO: 19, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at AAVS1 site 1/4 is shown in SEQ ID NO: 20, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at AAVS1 site 2 is shown in SEQ ID NO: 21, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at AAVS1 site 3 is shown in SEQ ID NO: 22, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at TRAC site 1 is shown in SEQ ID NO: 23, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at TRAC site 2 is shown in SEQ ID NO: 24, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at TRAC site 3 is shown in SEQ ID NO: 25, the mTurquoise2 sequence with 800 bp homology arms (HDR) site-directed integrated at B2M site 2 is shown in SEQ ID NO: 26, the CD19-CAR sequence with 200 bp homology arms (HDR) site-directed integrated at AAVS1 site 2 is shown in SEQ ID NO: 27, the CD19-CAR sequence with 400 bp homology arms (HDR) site-directed integrated at AAVS1 site 2 is shown in SEQ ID NO: 28, the CD19-CAR sequence with 800 bp homology arms (HDR) site-directed integrated at AAVS1 site 2 is shown in SEQ ID NO: 29, the CD19-CAR sequence with 200 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 30, and the CD19-CAR sequence with 400 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 31, the CD19-CAR sequence with 800 bp homology arms (HDR) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 32. The CD19-CAR sequence with 200 bp homology arms (HDR) site-directed integrated at TRAC site 2 is shown in SEQ ID NO: 33, the CD19-CAR sequence with 400 bp homology arms (HDR) site-directed integrated at TRAC site 2 is shown in SEQ ID NO: 34, the CD19-CAR sequence with 800 bp homology arms (HDR) site-directed integrated at TRAC site 2 is shown in SEQ ID NO: 35, the CD19-CAR sequence with 200 bp homology arms (HDR) site-directed integrated at B2M site 2 is shown in SEQ ID NO: 36, the CD19-CAR sequence with 400 bp homology arms (HDR) site-directed integrated at B2M site 2 is shown in SEQ ID NO: 37, the CD19-CAR sequence with 800 bp homology arms (HDR) site-directed integrated at B2M site 2 is shown in SEQ ID NO: 38.
Sequences of linear double-stranded DNA (DNA donor) as a comparative example are shown in any one of SEQ ID NO: 39-44.
Among them, the mTurquoise2 sequence with 800 bp homology arms (HITI-pb or writing“HITI (pb)”) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 39, the mTurquoise2 sequence with 800 bp homology arms (HITI) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 40, the mTurquoise2 sequence with 800 bp homology arms (MMEJ) site-directed integrated at PD1 site 1 is shown in SEQ ID NO: 41, the mTurquoise2 sequence with 800 bp homology arms (HITI-pb or writing“HITI (pb)”) site-directed integrated at PD1 site 2 is shown in SEQ ID NO: 42, the mTurquoise2 sequence with 800 bp homology arms (HITI) site-directed integrated at PD1 site 2 is shown in SEQ ID NO: 43, the mTurquoise2 sequence with 800 bp homology arms (MMEJ) site-directed integrated at PD1 site 2 is shown in SEQ ID NO: 44.
In the figures of this application, “Untreated T” refers to untreated T cells, “Control” refers to T cells electroporated only with homologous templates and Cas9, “LV-19bbz” refers to CD19-CART cells prepared by lentivirus, “AAVS1-19bbz” refers to non-viral AAVS1 site-directed integrated CD19-CART cells, and “PD1-19bz” refers to non-viral PD1 site-directed integrated CD19-CART cells.
The effect of DNA templates in the form of plasmid and linear double-stranded DNA on T cells was first compared. The results showed that the viability of cells was significantly higher than that of using plasmids when templates were linear double-stranded DNA (
Following this, the effect of homology arm length was compared. Recombination efficiency tests were first carried out at two PD1 sites using the fluorescent protein mTurquoise2 sequence as the exogenous sequence (
In previous experiments, we mainly explored and optimized the site-directed integration conditions for CD3+ T cells. On this basis, we attempted to edit CD4+and CD8+ T cells using the same approach. The results showed that our method had similar site-directed integration rates in CD3+, CD4+, and CD8+ T cells (
Using this method of the present invention, we successfully constructed AAVS1 site-directed integrated CD19-CART cells in different donor cells and verified them by sequencing, with an overall CAR positive rate of approximately 10%-20% and a knock-out rate of approximately 65%-90%, reflecting the robustness of cell preparation (
Using this method, we successfully constructed PD1 site-directed integrated CD19-CART cells in different donor cells and verified them by sequencing, with an overall CAR positive rate of approximately 10%-30% and a knock-out rate of approximately 80%-95%, reflecting the robustness of cell preparation (
In summary, AAVS1, PD1, TRAC, and B2M site-directed integrated CAR-T cells can be successfully constructed by the CRISPR/Cas9 gene editing tool using the present invention method combined with site selection. The present invention proves that the site-directed integrated CAR-T cells prepared by the method of the present invention have a higher positive rate and can function effectively when compared with the prior art. Compared with traditional lentiviral preparation methods, this technique can reduce the high cost caused by the use of viruses in the preparation of CAR-T, reduce the potential safety risks caused by random insertion when using viruses, and also improve the homogeneity of CAR-T products. In addition, this method can also be applied to construct diverse CAR-T cells and enhance the anti-tumor ability of CAR-T cells. This example proves the importance and value of the method of improving the site-directed integration of exogenous sequences in T cells protected by the present invention, but is not limited to the preparation of AAVS1, PD1, TRAC and B2M site-directed integrated CAR-T cells, which can be extended to the site-directed integration of exogenous sequences at other sites and the development of other T cell immunotherapies.
All references mentioned in this invention are cited in this application as references, just as each article is cited separately as references. It is also understood that, having read the foregoing lectures on the present invention, a skilled person in the art may make various modifications or modifications to the present invention in such equivalent form as would fall within the scope of the claims attached to this application.
Number | Date | Country | Kind |
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202010949701.5 | Sep 2020 | CN | national |
Filing Document | Filing Date | Country | Kind |
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PCT/CN2021/116531 | 9/3/2021 | WO |