Preparation method of cell nutrient solution for promoting hair regeneration
A nutrient solution and cell technology, which is applied in the field of human-derived cytokine hair growth nutrient solution and its preparation, can solve the problems of limited materials and inability to be used in clinical promotion, and achieve the effects of increasing survival, facilitating clinical promotion, and promoting cell secretion
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Embodiment 1
[0034] Step 1: Primary isolation of ADSCs
[0035] The adipose tissue obtained by liposuction was centrifuged at 1500r / min at 21°C for 5min, and the liquid part was removed to obtain solid fat particles. Then remove the connective tissue from the obtained fat particles, cut the large pieces of tissue with tissue scissors, add an equal volume of normal saline to wash, centrifuge at 1000r / min, 21°C for 10min, remove the liquid part, and obtain solid fat particles. Then add collagenase solution prepared with an equal volume of normal saline, 200U / ml, 37°C, constant temperature shaking and digestion for 60min, collect the digestive juice, centrifuge at 800r / min, 21°C for 10min, remove the supernatant, take the cell pellet, and then add 5ml of normal saline , 800r / min, centrifuge at 21°C for 10min, wash the cells, take the cell pellet, resuspend with 3ml of culture medium, count and count at 1×10 6 cells / flask inoculated at 75cm 2 culture flask at 37°C, 5% CO 2 Cultivate in a co...
Embodiment 2
[0043] Step 1: Primary isolation of ADSCs
[0044] The adipose tissue obtained by liposuction was centrifuged at 2000r / min at 21°C for 3min, and the liquid part was removed to obtain solid fat particles. Then remove the connective tissue from the obtained fat particles, cut the large pieces of tissue with tissue scissors, add an equal volume of normal saline to wash, centrifuge at 1500r / min, 21°C for 3min, remove the liquid part, and obtain solid fat particles. Then add collagenase solution prepared with an equal volume of normal saline, 200U / ml, 37°C, shake and digest at a constant temperature for 30min, collect the digestive juice, centrifuge at 1000r / min, 21°C for 8min, remove the supernatant, take the cell pellet, and then add 8ml of normal saline , 1000r / min, centrifuge at 21°C for 8min, wash the cells, take the cell pellet, resuspend with 5ml of culture medium, count and count at 1×10 6 cells / flask inoculated at 75cm 2 culture flask at 37°C, 5% CO 2 Cultivate in a con...
Embodiment 3
[0052] Step 1: Primary isolation of ADSCs
[0053] The adipose tissue obtained by liposuction was centrifuged at 1000r / min at 21°C for 10min to remove the liquid part to obtain solid fat particles. Then remove the connective tissue from the obtained fat particles, cut the large pieces of tissue with tissue scissors, add an equal volume of saline to wash, centrifuge at 1200r / min, 21°C for 5min, remove the liquid part, and obtain solid fat particles. Then add collagenase solution prepared with an equal volume of normal saline, 200U / ml, 37°C, shake and digest at a constant temperature for 45min, collect the digestive juice, centrifuge at 1200r / min, 21°C for 5min, remove the supernatant, take the cell pellet, and then add 10ml of normal saline , 1500r / min, centrifuge at 21°C for 5min, wash the cells, take the cell pellet, resuspend with 10ml of culture medium, count and count at 1×10 6 cells / flask inoculated at 75cm 2 culture flask at 37°C, 5% CO 2 Cultivate in a constant tempe...
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