Isolated culture method of alveolar type II epithelial cells of naked mole rats
A technique for the isolation and cultivation of epithelial cells, applied in cell dissociation methods, respiratory/lung cells, epidermal cells/skin cells, etc., can solve the problem of low purity of the primary isolation of naked mole rat alveolar epithelial type II cells, which is unfavorable for naked mole rats Mouse resistance to hypoxia and anti-tumor research, low affinity and other issues
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Embodiment 1
[0039] Embodiment 1 Naked mole rat alveolar type II epithelial cell isolation and culture method
[0040] (1) After killing an adult naked mole rat by decapitation, soak it in 75% ethanol for 5 minutes, remove the whole lung tissue as soon as possible in an ultra-clean bench, rinse the lung tissue with pre-cooled washing solution until clear, and cut the lung tissue into 1mm 3 Small pieces, transferred into a penicillin vial.
[0041] (2) Add 2mL of tissue digestion solution and digest at 35°C for 5min. Remove the digested cell suspension, add an equal volume of inhibitor solution to the tissue digestion solution to terminate the digestion;
[0042] (3) Repeat step (2) 5 times until the tissue blocks basically disappear. Combine 20 mL of the cell suspension, filter through a 200-mesh cell sieve, collect the filtrate, and centrifuge at 100 g for 5 min to collect the cells;
[0043] (4) Resuspend the cells in 5ml adhesion medium preheated at 35°C, and insert them into a 10cm...
Embodiment 2 Embodiment 1
[0045] Example 2 Cell Identification, Purity and Vitality Evaluation of Alveolar Type II Epithelial Cells of Example 1
[0046] 1. Cell identification
[0047] ①Pro-SP-C immunofluorescence staining identification
[0048] SP-C is an alveolar surfactant protein specifically expressed by alveolar type II epithelial cells, while the other three surfactant proteins SP-A, SP-B, and SP-D are also expressed in other cells, so SP among the surfactant proteins was selected. -C can be used to identify alveolar type II epithelial cells.
[0049] When alveolar type II epithelial cells reach the ideal density, fix the sample with 4% (W / V) paraformaldehyde for 10 minutes; wash with PBS for 5 minutes, and treat with 0.1% (V / V) Triton X-100 for 10 minutes to increase the permeability of the cell membrane ; goat serum was blocked for 1 h; incubated with primary antibody (SFTPC was diluted with PBS containing 0.1% (V / V) Triton X-100 1:1000) and diluted overnight at 4°C; in addition, PBS was u...
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