High-efficiency genetic transformation method for soybean immaturity seed lobe regeneration system with auxiliary vacuum permeation
A genetic transformation method and vacuum infiltration technology are applied in the field of high-efficiency genetic transformation of improving soybean genetic traits and vacuum infiltration-assisted soybean immature cotyledon regeneration system, so as to achieve the effects of improving infection efficiency, increasing invasion opportunity and increasing transformation rate.
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Embodiment 1
[0029] Jilin 35 somatic embryogenesis and introduction of exogenous genes
[0030] Jilin 35 was planted in the field, and young soybean pods of 16-20 days after flowering were picked, rinsed once with sterile water, soaked in 75% ethanol for 2 minutes, and rinsed with sterile water for 3 times. Peel off the seed coat, select 3-5mm cotyledons to remove the hypocotyl, and inoculate the cotyledons with the adaxial side up in MS medium + 2,4-D 20mg / L + sucrose 3.0g / L + plant gel 3.0g / L (pH=6.0 ) in the dark at 25°C for 14-30 days.
[0031] Select bright and spherical green embryoid bodies, and move to MS medium + 2,4-D 5.0 mg / L + asparagine 1.0 g / L + sucrose 3.0 g / L + plant gel 3.0 g / L (pH=5.8 ), cultivated under light at 25°C (16hr / 8hr), and subcultured once every two weeks.
[0032] The somatic embryos were transferred to MS medium + activated carbon 4.0g / L + maltose 60.0g / L + phytogel 3.0g / L (pH=6.4), and cultured under light at 25°C (16hr / 8hr). Passage every two weeks.
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Embodiment 2
[0038] Somatic Embryogenesis and Introduction of Foreign Genes in Jilin 47
[0039] Jilin 47 was planted in the field, and young soybean pods that had bloomed for 16-20 days were picked, rinsed once with sterile water, soaked in 75% ethanol for 2 minutes, and rinsed three times with sterile water. Peel off the seed coat, select 3-5mm cotyledons to remove the hypocotyl, and inoculate the cotyledons with the adaxial side up in MS medium + 2,4-D 40mg / L + sucrose 3.0g / L + plant gel 3.0g / L (pH=6.0 ) in the dark at 25°C for 14-30 days.
[0040] Select bright and spherical green embryoid bodies, and move to MS medium + 2,4-D 5.0 mg / L + asparagine 1.0 g / L + sucrose 3.0 g / L + plant gel 3.0 g / L (pH=5.8 ), cultivated under light at 25°C (16hr / 8hr), and subcultured once every two weeks.
[0041] The somatic embryos were transferred to MS medium + activated carbon 4.0g / L + maltose 60.0g / L + phytogel 3.0g / L (pH=6.4), and cultured under light at 25°C (16hr / 8hr). Passage every two weeks....
Embodiment 3
[0047] Somatic Embryogenesis and Introduction of Foreign Genes in Jilin 20
[0048] Jilin 20 was planted in the field, and young soybean pods that had bloomed for 16-20 days were picked, washed once with sterile water, soaked in 75% ethanol for 2 minutes, and rinsed three times with sterile water. Peel off the seed coat, select 3-5mm cotyledons to remove the hypocotyl, and inoculate the cotyledons with the adaxial side up in MS medium + 2,4-D 30mg / L + sucrose 3.0g / L + plant gel 3.0g / L (pH=6.0 ) in the dark at 25°C for 14-30 days.
[0049] Select bright and spherical green embryoid bodies, and move to MS medium + 2,4-D 5.0 mg / L + asparagine 1.0 g / L + sucrose 3.0 g / L + plant gel 3.0 g / L (pH=5.8 ), cultivated under light at 25°C (16hr / 8hr), and subcultured once every two weeks.
[0050] The somatic embryos were transferred to MS medium + activated carbon 4.0g / L + maltose 60.0g / L + phytogel 3.0g / L (pH=6.4), and cultured under light at 25°C (16hr / 8hr). Passage every two weeks....
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