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A kind of preparation method of neuron cryopreservation liquid

A technology of neuron and cryopreservation solution, which is applied in the field of preparation of neuron cryopreservation solution, and can solve the problem of low recovery rate of neuron cryopreservation

Active Publication Date: 2021-12-14
BEIJING TIANTAN HOSPITAL AFFILIATED TO CAPITAL MEDICAL UNIV
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0005] Aiming at the problem that the traditional cryopreservation method cannot avoid the low survival rate and poor activity of neuron cryopreservation, the invention provides a preparation method of neuron cryopreservation solution

Method used

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  • A kind of preparation method of neuron cryopreservation liquid
  • A kind of preparation method of neuron cryopreservation liquid
  • A kind of preparation method of neuron cryopreservation liquid

Examples

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preparation example Construction

[0031] The present invention also provides a method for preparing a neuron cryopreservation solution, comprising the following steps:

[0032] Sampling: Take the isolated mammalian nervous tissue, shred it and place it in the first centrifuge tube for 4-6 minutes at 800-1200rpm, and remove the centrifuged supernatant;

[0033] Digestion: Add trypsin to the first centrifuge tube, blow off the precipitated cells in the first centrifuge tube, draw out the precipitated cells and place them in the digestion culture dish, add trypsin to the digestion culture dish, place the digestion culture dish at 37 After 8-12 minutes in the incubator at ℃, add the planting medium to the digestion culture dish to terminate the digestion;

[0034] Preparation of cell suspension: Filter the mixture in the digestion dish through a cell sieve, centrifuge at 800-1200rpm for 4-6min, remove the supernatant after centrifugation, and obtain primary neurons;

[0035] Cryopreservation: mix the primary neur...

Embodiment 1

[0058] (1) Experimental preparation: Coat four 24-well plates and two 6-well plates with poly-lysine, remove the coating solution after staying overnight at 37°C, blow it for 2 hours until dry; wash with sterile water twice, add sugar Type DMEM medium 0.3mL / well, remove the DMEM medium before cell planting, replace the 24-well plate with 500μL planting medium, and replace the 6-well plate with 2mL planting medium; sterilize surgical instruments, including scissors, tweezers and fiber tweezers .

[0059] (3) Disinfect the microscope, and anesthetize the animal to be tested in this implementation—the 5-day-old embryonic mouse.

[0060] (4) Sampling: Cut open the skull of the embryonic mouse, take out the brain tissue, peel off the blood vessels and meninges in ice-cold DMEM medium, cut the brain tissue into pieces, take out the brain tissue, put it in a 15mL first centrifuge tube and centrifuge at 1000rpm for 5min, remove Centrifuge the supernatant.

[0061] (5) Digestion: Add...

Embodiment 2

[0073] The difference between Example 2 and Example 1 is that in the recovery step, the frozen neurons are transferred to the recovery medium for culture. The proportioning ratio of the planting medium, neuron medium, neural stem cell medium, cryopreservation solution, and recovery medium used in Example 2 is as follows:

[0074] Volume ratio of planting medium components: 41.70mL DMEM, 5.00mL HS, 3.00mL FBS, 0.30mL double antibody.

[0075] Volume ratio of neuron medium components: 50.00mL Neurobasal A, 1.00mL B27, 0.30mL double antibody.

[0076] Volume ratio of neural stem cell medium components: 45.00mL DMEM / F12, 1.00mLbFGF, 1.00mLEGF, 1.00mLB27, 0.50mLN2, 0.50mL double antibody.

[0077] The volume ratio of the cryopreservation solution components: 50.00mL neuron culture medium, 45.00mL 10% bovine serum albumin, 5.00mL dimethyl sulfoxide.

[0078] Volume ratio of recovery medium components: 50.00mL neuron medium, 50.00mL neural stem cell medium, 1.0mL 10% BSA and 1.0mL ...

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Abstract

The invention discloses a preparation method of a neuron cryopreservation solution, which comprises the following steps: sampling, digestion, cell suspension preparation, freezing storage and recovery steps; neither the neuron cryopreservation solution nor the medium used contain glutamine amides. In the preparation method of the above-mentioned neuron cryopreservation solution, primary neurons are mixed with the cryopreservation solution of the present invention before cryopreservation, which can reduce the damage of neuron cryopreservation, and the survival rate of neurons after recovery is high and the activity is strong. Furthermore, the method for sampling and separating nerve tissue of the present invention is quick and convenient, avoids neuron damage and cell contamination, improves sampling efficiency and facilitates subsequent digestion and processing.

Description

technical field [0001] The invention belongs to the technical field of tissue cell culture, and in particular relates to a preparation method of a neuron cryopreservation solution. Background technique [0002] In the study of the nervous system, the primary isolation and culture of neurons is a very important in vitro study, which is used to study various physiological functions of nerve cells. Due to the limitation of obtaining nerve tissue, the primary isolation of neurons is mainly in on rodent mammals. For example, rodents commonly used for primary isolation of neurons include fetal mice and neonatal mice. However, due to the lack of proliferative ability of neuron cells, after primary isolation, it is not suitable for long-term survival, growth, and differentiation in vitro, which is not conducive to the smooth progress of research; in addition, primary neurons are particularly sensitive to the external environment. It is very easy to die after adverse stimulation, s...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): A01N1/02
CPCA01N1/0221
Inventor 郭安臣王群王拥军
Owner BEIJING TIANTAN HOSPITAL AFFILIATED TO CAPITAL MEDICAL UNIV