Fish high-fat storage hepatocyte separation and culture method

A culture method and hepatocyte technology are applied in the field of fish high-fat storage hepatocyte isolation and culture, which can solve the problems of long modeling time, limited application of primary mature cell culture, difficulty in primary cell isolation and culture, etc. Effects of isolation and culture difficulties

Active Publication Date: 2020-10-30
GUANGDONG LAB ANIMALS MONITORING INST
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

So far, the methods for cell culture mainly contain the following: tissue block adherent culture method (Wu Ning, Wu Chenglong. (2007)), mixed culture method (Bhatia, S.N., Balis, U.J., (1999). The FASEBjournal ), single-layer collagen culture method, co-culture system, etc., the above-mentioned commonly used primary mature cell culture can only maintain the shape and function of the cells within 1-2 weeks, and then gradually degenerate and die, so that the primary mature cell culture App is restricted
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Method used

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  • Fish high-fat storage hepatocyte separation and culture method
  • Fish high-fat storage hepatocyte separation and culture method
  • Fish high-fat storage hepatocyte separation and culture method

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Embodiment 1

[0024] (1) Select 50-day-old goby juveniles, and obtain their liver tissue under sterile conditions. The liver tissue block is slowly rinsed three times with sterile PBS, placed in the middle of a cell sieve with a pore size of 50 μm, and the tissue block is separated with a sterile instrument. Disperse into 1±0.1mm 2 Small piece;

[0025] (2) Place a cell sieve with a pore size of 50 μm on top of a cell sieve with a pore size of 20 μm, and the cell sieve with a pore size of 20 μm is located in M199 medium (Gibco.Lot: 2044485) containing 10% FBS by volume;

[0026] (3) Rinse the upper and lower layers of cell sieves with serum-free M199 medium first, slowly and continuously drip trypsin solution with a mass fraction of 0.25% on the tissue block, flow and continue to digest until the tissue block disappears;

[0027] (4) Collect the cells on the 20 μm cell sieve, the cell size is 20 μm to 50 μm, wash slowly and gently for 3 times with 10% FBS by volume fraction, and count;

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Abstract

The invention discloses a fish high-fat storage hepatocyte separation and culture method. The method comprises the following steps: a, selecting 45-55d young gobius giurinus, obtaining liver tissues of the young gobius giurinus under a sterile condition, and dispersing the liver tissues into blocks to obtain tissue blocks; b, putting the cell sieve with the pore diameter of 20 microns into a trypsin stop solution, and arranging the cell sieve with the pore diameter of 50 microns above the cell sieve with the pore diameter of 20 microns; c, putting the tissue blocks into a cell sieve with the pore diameter of 50 microns, continuously adding trypsin liquid into the cell sieve with the pore diameter of 50 microns to digest the tissue blocks, continuously digesting by flowing, collecting cellson the cell sieve with the pore diameter of 20 microns, and cleaning with 10% FBS to obtain high-fat storage liver cells; and d, inoculating the high-fat storage hepatocytes into a culture medium forculturing. The high-fat storage hepatocytes can be stabilized for one week after adherence, adipose cells can survive for about one month, and the high-fat storage hepatocytes can be used for cell level experiments in the period so that the problem that mature fish adipose cells are difficult to separate and culture is solved.

Description

technical field [0001] The invention relates to the field of cell biology, in particular to a method for separating and culturing fish high-fat storage hepatocytes. Background technique [0002] In scientific research, in order to further verify the accuracy and authenticity of experimental results, verification experiments at the cell level are generally required, and the sources of cells used at the cell level are commercialized cells and primary cell culture. Primary cell culture is the first culture in vitro of cells obtained from donor living tissue, allowing them to grow and multiply continuously under artificial conditions. The cells at this time maintain the basic properties of the original cells, which is the basis of various experimental studies and the first step in establishing various cell lines. Primary cell culture includes differentiated primary stem cell culture and primary mature cell culture; the key to culturing cells in vitro is how to separate cells wi...

Claims

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Application Information

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IPC IPC(8): C12N5/071
CPCC12N5/067C12N2509/00Y02A40/81
Inventor 苗宗余蔡磊黄韧李建军魏远征叶惠欣曾进
Owner GUANGDONG LAB ANIMALS MONITORING INST
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