Vitrification freezing and storing method of a little somatic cells for cloning domestic animal
A vitrification and preservation method technology, applied in the preservation of human or animal bodies, biochemical equipment and methods, applications, etc., can solve the problems of easy loss of small particles, large equipment costs, waste of cells, etc., and achieve the effect of cryopreservation Good, low cost, high survival rate
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Embodiment 1
[0019] The steps for vitrification and cryopreservation of bovine ear fibroblasts are as follows:
[0020] (1), configuration liquid:
[0021] Base solution: add 20ml fetal bovine serum (V / V) and 0.5ml antibiotic solution (Antibiotic-Antimycotic) to 100ml cell culture medium (DMEM solution);
[0022] Vitrification solution I: add 2ml ethylene glycol (V / V) and 2ml dimethyl sulfoxide (V / V) to 100ml base solution;
[0023] Vitrification solution II: Add 30ml of ethylene glycol (V / V), 30ml of dimethyl sulfoxide (V / V) and 0.2 mole of trehalose to 100ml of base solution;
[0024] Thawing solution: Add 0.25 moles of sucrose to 100ml base solution;
[0025] (2), Freezing: Cultivate cells with 6-well culture plate, digest cells in 1 hole when the confluence of cells is 85%, collect cell suspension with 1.5 ml centrifuge tube, centrifuge at 1000g for 5 minutes, and remove supernatant. Then add 1 ml of Vitrification Solution I, centrifuge at 1000 g for 5 minutes, and remove the supern...
Embodiment 2
[0029] The steps of vitrification cryopreservation of frozen bovine fallopian tube epithelial cells are as follows:
[0030] (1), configuration liquid:
[0031] Base solution: add 30ml fetal bovine serum (V / V) and 1.5ml antibiotic solution (Antibiotic-Antimycotic) to 100ml cell culture medium (DMEM solution);
[0032] Vitrification solution I: add 4ml ethylene glycol (V / V) and 4ml dimethyl sulfoxide (V / V) to 100ml base solution;
[0033] Vitrification solution II: add 35ml of ethylene glycol (V / V), 35ml of dimethyl sulfoxide (V / V) and 0.3 mole of trehalose to 100ml of base solution;
[0034] Thawing solution: Add 0.35 moles of sucrose to 100ml base solution;
[0035] (2), Freezing: Cultivate cells with 6-well culture plates, digest cells in 1 hole when the confluence of cells is 80%, collect cell suspension with 1.5 ml centrifuge tube, centrifuge at 800g for 5 minutes, and remove supernatant. Then add 1 ml of Vitrification Solution I, centrifuge at 800 g for 5 minutes, and ...
Embodiment 3
[0039] The steps of vitrification cryopreservation of frozen goat fallopian tube epithelial cells are as follows:
[0040] (1), configuration liquid:
[0041] Base solution: Add 25ml of fetal bovine serum (V / V) and 1ml of antibiotic solution (Antibiotic-Antimycotic) to 100ml of cell culture medium (DMEM solution);
[0042] Vitrification solution I: add 3ml ethylene glycol (V / V) and 3ml dimethyl sulfoxide (V / V) to 100ml base solution;
[0043] Vitrification solution II: Add 30ml of ethylene glycol (V / V), 30ml of dimethyl sulfoxide (V / V) and 0.25 mole of trehalose to 100ml of base solution;
[0044] Thawing solution: add 0.3 mole of sucrose to 100ml base solution;
[0045] (2), Freezing: Cultivate cells with 6-well culture plate, digest cells in 1 hole when the degree of cell confluence is 80%, collect cell suspension with 1.5 ml centrifuge tube, centrifuge at 900g for 7 minutes, and remove supernatant. Then add 1 ml of Vitrification Solution I, centrifuge at 900 g for 7 minu...
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