Tumor infiltrating lymphocytes separation method

A lymphocyte and tumor infiltration technology, applied in the field of cell separation, can solve the problems of reducing the activity of TIL cells, manpower and material resources, etc., and achieve the effect of high survival rate, specific and efficient anti-tumor activity, and simple survival rate

Inactive Publication Date: 2015-07-08
ZHEJIANG UNIV
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  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0004] At present, most TILs are separated by mechanical methods or enzymatic digestion methods, which not only cost a lot of manpower and material resources, but also reduce the cell activity of TILs after separation.

Method used

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Examples

Experimental program
Comparison scheme
Effect test

specific Embodiment 1

[0030] 1. Isolation of tumor infiltrating lymphocytes

[0031] (1) After washing the liver cancer tumor tissue block with PBS buffer solution, place it in a culture dish, add 5 times the volume of trypsin digestion solution and soak for 3 hours;

[0032] (2) Trim the soaked tumor tissue block to 0.5mm 3 After granulation, put the culture dish in a 37°C water-bath shaker, incubate the tumor tissue with trypsin digestion solution for 1 hour, so that the tumor tissue block can be fully digested and dispersed; collect the cell suspension and pass it through a 200-mesh metal filter , separate and collect single cells into a 50ml centrifuge tube; wash the culture dish twice with trypsin digestion solution, and transfer all the liquid to the 50ml centrifuge tube;

[0033] (3) Place the 50ml centrifuge tube from the previous step on ice for 10 minutes, then centrifuge it in a 50g centrifuge for 2 minutes; discard the bottom sediment, transfer the supernatant to another 50ml centrifug...

specific Embodiment 2

[0041]Compared with Example 1, in this example: the separation object is a lung cancer tumor tissue piece; the addition amount of trypsin digestion solution in step (1) is 10 volume times; the incubation time in water bath shaker in step (2) is 2 Hour; The mass ratio of the density gradient centrifugate added in step (4) and cell suspension is 1:2; All the other contents are the same as in Example 1.

specific Embodiment 3

[0042] Compared with Example 1, in this example: the separation object is a gastric cancer tumor tissue block; the amount of trypsin digestion solution in step (1) is 7 volume times; the incubation time in a water bath shaker in step (2) is 1.5 Hour; The mass ratio of the density gradient centrifugate added in the step (4) and the cell suspension is 1:1.5; All the other contents are the same as in Example 1.

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PUM

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Abstract

The invention relates to a cells separating technology, and provides a tumor infiltrating lymphocytes separation method. The method is characterized by adding tumor tissue masses in a trypsin-EDTA solution for immersion and incubation, fully digesting and dispersing the tumor tissue masses; separating and collecting single cell and being resuspended by the trypsin-EDTA solution for multitime density gradient centrifugation, incubating and separating by an erythrocyte lysate, using calf serum-containing PBS buffer or resuspending to obtain the dissolved tumor infiltrating lymphocytes. In the invention, an enzymatic digestion method and a machinery method are combined for dual separating the enzymatic digestion with high efficiency, compared with the machinery method or the enzymatic digestion method, the survival rate of the obtained tumor infiltrating lymphocytes is high, and the method is simple and easy to operate. The obtained tumor infiltrating lymphocytes can be massively propagated through in vitro stimulation of interleukin 2 (1L-2), have antineoplastic activity with specialty and high efficiency, and provides powerful basis and new approach for treating tumour.

Description

technical field [0001] The invention belongs to cell separation technology, and relates to a method for separating tumor infiltrating lymphocytes. Background technique [0002] In 1986, Rosenberg et al. first reported lymphocytes isolated from mouse solid tumors, called "tumor infiltrating lymphocytes (TIL)", which are mainly T cells that mainly exist in the tumor stroma. A heterogeneous population of lymphocytes, mostly clustered around the tumor or in the stroma surrounding the cancer nest. Further studies have found that this kind of cells can proliferate in large quantities after being stimulated by interleukin 2 (IL-2) in vitro, and has a strong effect of specifically killing tumor cells, and its anti-tumor effect is better than that of lymphokine-activated killer cells ( Lymphokine activated killer cell, LAK) is 50-100 times higher. For example, studies have found that TILs from melanoma patients only have killing activity on autologous tumor cells, but not on autolo...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N5/0783
Inventor 吴健曹林平陈康杰丁超峰
Owner ZHEJIANG UNIV
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