Culture method for functionally enhanced TILs

A culture method and enhanced technology, applied in the field of biomedicine, can solve the problems of tumor immune escape, limit the wide application of TIL cell therapy, affect the anti-tumor activity of TIL cells, etc., and achieve the effect of improving the activity and strongly killing the activity of tumor cells.

Pending Publication Date: 2020-03-31
SUN YAT SEN UNIV CANCER CENT
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0005] Due to the limited source of TIL cells, conventional TIL cell culture methods are affected by various factors such as tumor size, the number of TIL cell infiltration in the tumor, and easy contamination during the process of taking tumor tissue, which limits the application of TIL cell therapy in clinical tumor treatment. widely used
Compared with cytokine-induced killer cells (CIK cells) and NK cells, the cell proliferation rate and proliferation rate during TIL cell culture are not as good as the former; and a large amount of IL-2 is required during the culture process, which can promote CD4+CD25+ regulatory Expansion of T lymphocytes, thereby affecting the anti-tumor activity of TIL cells, leading to the occurrence of tumor immune escape

Method used

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  • Culture method for functionally enhanced TILs
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  • Culture method for functionally enhanced TILs

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0028] Example 1: Cultivation of function-enhanced TIL cells

[0029] The invention provides a method for cultivating function-enhanced TIL cells. According to different stages of cell culture, the starting medium, induction medium, expansion medium and function-enhancing medium are sequentially used. Described cultivation method comprises the following steps:

[0030] 1) Start-up culture stage: Collect tumor tissue to separate infiltrating lymphocytes, cut tumor tissue into small pieces in a culture dish, centrifuge at room temperature at 1800rpm for 8 minutes, discard supernatant, add 10ml IV collagenase solution and blow evenly; place in 37℃ water bath for 2 hours for digestion ; Collect the supernatant after digestion, pass through a 100 μm sterile sieve; wash twice with normal saline (centrifuge at room temperature at 1800 rpm for 8 minutes, discard the supernatant), take the precipitate and suspend it with X-VIVO, and carry out Ficoll gradient with lymphocyte separation ...

Embodiment 2

[0045] Example 2: Comparison of the killing function of TIL cells that have undergone a function-enhanced culture stage (function-enhanced TIL) and TIL cells that have not undergone a function-enhanced culture stage (common TIL cells) on lung cancer cells.

[0046] Function-enhanced TIL cells were obtained by culturing for 14 days or 15 days through the steps of separating lymphocytes from lung cancer tumor tissue, starting culture phase, induction culture phase, expansion culture phase, and function enhancement culture phase. Common TIL cells were obtained by culturing lymphocytes from lung cancer tumor tissue, starting culture phase, induction culture phase, and expansion culture phase; on the 14th day of culture, the function-enhanced TIL cells and common TIL cells were collected respectively, and the following procedures were performed: Kill experiment.

[0047] The lung cancer cell lines A549 and H209 stably expressing green fluorescent protein (GFP) were mixed with norma...

Embodiment 3

[0049] Example 3: Comparing the secretion levels of cytokines between TIL cells that have undergone a function-enhanced culture phase (function-enhanced TIL) and TIL cells that have not undergone a function-enhancement culture phase (common TIL)

[0050] Function-enhanced TIL cells were obtained by culturing lymphocytes from lung cancer tumor tissue, starting culture phase, induction culture phase, expansion culture phase, and function enhancement culture phase. Ordinary TIL cells are obtained through the steps of separation of lymphocytes from lung cancer tumor tissue, start-up culture stage, induction culture stage, expansion culture stage and other steps. On the 14th day of culture, the function-enhanced TIL cells and ordinary TIL cells were collected respectively, and the ability of the two kinds of cells to secrete cytokines was detected by flow cytometry and ELISA respectively.

[0051] The lung cancer cell lines A549 and H209 stably expressing green fluorescent protein ...

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Abstract

The invention discloses a culture method for functionally enhanced tumor infiltrating lymphocytes (TILs). The method includes the following steps: separating lymphocytes from tumor tissue, adding a start culture medium, performing inoculation in a 12-well culture plate (4 ml / well), performing start lymphocyte culture for 10 days or 14 days to obtain start TILs, and performing cryopreservation on the obtained start TILs for standby application; suspending the lymphocytes in a 25 cm<2> culture flask (20 ml / flask) by using an induction culture medium, placing the culture flask in an incubator having 5% CO2 at 37 DEG C, and performing TIL induction culture for 1 day; performing half quantity change by using an expansion culture medium, and performing expansion flask culture and expansion bag culture for 13 days or 14 days; on the 14th or 15th day of culture, collecting TILs, performing washing by using normal saline, and resuspending the TILs by using a function enhancement culture medium,and performing incubation for 30 min; and collecting TILs, and performing functional test to obtain the functionally enhanced TILs. The culture method described in the invention can obtain the functionally enhanced TILs with stronger tumor cell killing activity and higher-level anti-tumor cytokine secretion ability.

Description

technical field [0001] The invention belongs to the field of biomedicine and relates to a cell culture method, in particular to a function-enhanced tumor infiltrating lymphocyte (Tumor infiltrating lymphocytes, TIL) cell culture method. Background technique [0002] Tumor immunotherapy is expected to become a new weapon to cure tumors, especially the application of anti-PD-1 antibody, anti-PD-L1 antibody and anti-CTLA-4 antibody in clinical tumor immunotherapy has received extensive attention, and they significantly prolong the life expectancy of advanced tumors. Survival for patients with malignant melanoma, lung and colon cancers, among others, is showing light for many patients with difficult-to-treat cancers. Immune checkpoint blockers mainly block T cell inhibitory signaling pathways in tumor tissue, thereby continuously activating T cells, breaking through the immune suppression of the tumor microenvironment, and achieving the purpose of killing tumor cells. 2018 is a...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N5/0781C12N5/0783
CPCC12N5/0635C12N5/0636C12N5/0646C12N2501/2302C12N2501/51C12N2501/515
Inventor 夏建川潘求忠何佳宋梦佳
Owner SUN YAT SEN UNIV CANCER CENT
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