An Improved Primary Culture Method of Hippocampal Neurons
A hippocampal neuron, primary culture technology, applied in the field of hippocampal neuron isolation and primary culture methods and reagents, can solve the problems of easy to increase bacterial contamination, lack of suitable, difficult to obtain, etc., to improve in vitro survival rate and digestion efficiency. Improve and increase the effect of physiological breathing
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Embodiment 1
[0041] The Bifidobacterium adolescentis LJM-001 of the present invention has been in the General Microbiology Center of China Microbiological Culture Collection Management Committee on August 17, 2010, which is referred to as CGMCC (Address: No. 1 Beichen West Road, Chaoyang District, Beijing) No. 3 Institute of Microbiology, Chinese Academy of Sciences, Zip code 100101) is preserved, and the classification is named Bifidobacterium adolescentis (Bifidobacterium adolescentis), and the preservation number is CGMCCNo.4090.
[0042] The Bifidobacterium adolescentis LJM-001 of the present invention is isolated from the feces of a healthy young man in Zhejiang Province.
[0043] Bifidobacterium adolescentis LJM-001 strain of the present invention has the following microbiological characteristics:
[0044] (1) Colony morphology: The colonies of the LJM-001 strain on the plate are off-white or milky white, opaque, shiny, smooth, raised, soft in texture, with neat edges, and a diameter...
Embodiment 2
[0051] Reagent purchase:
[0052] DMEM / F12 neural basal medium, Neurobasal medium and B 27 Purchased from Gibco Company; polylysine, fetal bovine serum (FBS), trehalose and L-glutamine were purchased from Sigma Company of the United States; penicillin and streptomycin mixed solution (double antibody) was purchased from HyClone Company of the United States.
[0053] Reagent configuration:
[0054] (1) The D-Hank's solution is obtained through the following steps: NaCl8.0g, KCl0.4g, NaCl 2 HPO 4 12H 2 O0.12g, KH 2 PO 4 0.06g, NaHCO 3 0.35g; Dissolve each component in approximately 500mL triple-distilled water and mix well, add triple-distilled water to make up to 1000mL, adjust the pH value to 7.2-7.4, subpackage, autoclave, subpackage, and store at 4°C for later use.
[0055] (2) The rinse liquid is obtained through the following steps: dissolve 2g trehalose, 3g glucose and 10mL double antibody in 100mL D-Hank's solution, mix well, add D-Hank's solution to 1000mL, 0.4 D...
Embodiment 3
[0066] The method for separating and primary culture of SD rat hippocampal neurons comprises the following steps:
[0067] Use the reagents prepared in Example 1 and Example 2 and configure the reagents.
[0068] (1) Rinsing: Take the hippocampus tissue of the isolated mammal, put it in the rinsing solution in an ice bath, remove red blood cells, capsules and connective tissue, and rinse it 2 to 5 times with the rinsing solution;
[0069] (2) Digestion: cut the hippocampal tissue rinsed in step 1 into a diameter of 1mm 3 For small pieces, use 5 times the tissue volume of digestion solution at 37°C for 5-10 minutes to organize into a porridge-like shape, stop digestion with cell seeding solution, and gently pipette until the tissue piece is 10 times to disperse the cells.
[0070] (3) Preparation of cell suspension: Collect the initial cell suspension after digestion in step 2, filter through a 200-mesh cell sieve, centrifuge at 800-1000 rpm at 4°C for 5-10 minutes, discard the ...
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