Culture medium for tissue culture of medicago ruthenica
A technology of tissue culture and culture medium, applied in the field of plant tissue culture, can solve the problems of low yield per unit area, achieve the effect of increasing the speed of culture, speeding up the speed of reproduction, and easy operation
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Embodiment 1
[0023] The petioles of lentils with robust growth were selected as explants, and the explants were sterilized.
[0024] The sterilized explants were inoculated into the induction medium for callus culture, and the culture period was 12 days, the temperature was 20° C., and the humidity was 60%. The formula of the induction medium was: MS+0.18mg / L 6 -BA+0.48mg / L NAA+0.18mg / L 2,4-D+0.45g / L CH.
[0025] Preferably, the explant size is 0.27 mm.
[0026] Preferably, the disinfection method is as follows: 75% alcohol disinfection for 25s, mercuric solution disinfection for 2min, and finally using sterile water to wash for 4 times, each rinse for 25s.
[0027] The induction rate was measured, and the specific data are shown in Table 1.
Embodiment 2
[0029] The petioles of lentils with robust growth were selected as explants, and the explants were sterilized.
[0030] The sterilized explants were inoculated into the induction medium for callus culture, and the culture period was 17 days, the temperature was 28° C., and the humidity was 80%. The formula of the induction medium was: MS+0.22mg / L 6 -BA + 0.53 mg / L NAA + 0.22 mg / L 2,4-D + 0.55 g / L CH.
[0031] Preferably, the explant size is 0.30 mm.
[0032] Preferably, the disinfection method is as follows: 75% alcohol disinfection for 35s, mercuric solution disinfection for 4 minutes, and finally 6 times of sterile water cleaning, each rinse for 35s.
[0033] The induction rate was measured, and the specific data are shown in Table 1.
Embodiment 3
[0035] The petioles of lentils with robust growth were selected as explants, and the explants were sterilized.
[0036] The sterilized explants were inoculated into the induction medium for callus culture, and the culture period was 15 days, the temperature was 25° C., and the humidity was 70%. The formula of the induction medium was: MS+0.20mg / L 6 -BA + 0.50 mg / L NAA + 0.20 mg / L 2,4-D + 0.50 g / L CH.
[0037] Preferably, the explant size is 0.28 mm.
[0038] Preferably, the disinfection method is as follows: 75% alcohol disinfection for 30s, mercuric solution disinfection for 3 minutes, and finally using sterile water to wash for 5 times, each rinse for 30s.
[0039] The induction rate was measured, and the specific data are shown in Table 1.
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