[Objective] The paper aims to optimize the abduction and domestication conditions of Taxus chinensis var.Mairei callus.[Method] We compared the efficiencies of callus between different explants and investigated the mu...[Objective] The paper aims to optimize the abduction and domestication conditions of Taxus chinensis var.Mairei callus.[Method] We compared the efficiencies of callus between different explants and investigated the multiplication conditions of callus and suspended cell culture conditions with the buds,young stems and young leaves from T.chinensis var as the explants.[Results] The effect was the best with the bud as the explants; the best way for sterilizing the explants of T.chinensis var mairei was:streptomycin detergent for 2 h + suds for 3 h + 75% alcohol disinfection for 30 s + 10% sodium hypochlorite solution for 25 min + 1‰ mercury chloride for 10 min; the optimum formula of callus subculture was:B5 + 4.0 mg/L NAA + 0.5 mg/L 2,4-D + 0.2 mg/L GA + 0.5 mg/L 6-BA + 2 g/L AC.[Conclusion] This research built the high efficient regeneration system of T.chinensis var.展开更多
Byrsonima intermedia A. Juss. is a species from the Brazilian Cerrado that produces edible fruits and, in common with other species from the Byrsonima genus, has pharmacological potential. Previous attempts to propaga...Byrsonima intermedia A. Juss. is a species from the Brazilian Cerrado that produces edible fruits and, in common with other species from the Byrsonima genus, has pharmacological potential. Previous attempts to propagate the species through conventional methods showed difficulties. Thus, the purpose of this work was to characterize pro-embryogenic masses of Byrsonima intermedia callus, aiming for their in vitro propagation through somatic embryogenesis. Leaf segments from in vitro germinated seedlings were employed as explants for callus production. The calli were then subcultured and exposed to dyes to fulfill their embryogenic potential. Digitalizations of the cytological preparations were made in order to measure the area that was stained by both Aceto-Carmine and Evans-Blue, using image tool software. Somatic embryos were induced after treatments with l-naphthaleneacetic acid (NAA). The percentages of double-colored areas (by Aceto-Carmine and Evans-Blue) were calculated and the data were analyzed by using the Skott-Knott test (P ≤ 0.05) and, the embryogenic callus, as well as the formation of somatic embryos were analyzed by using the Krsuskal-Wallis rank test (P ≤0.05). The results show that double coloration is effective at identifying cells showing embryogenic potential. Early callus subculture phases show a larger percentage ofembryogenic area (83%) Somatic embryos were induced by using high auxin level.展开更多
基金Supported by National College Student Innovative Plan(091030719)~~
文摘[Objective] The paper aims to optimize the abduction and domestication conditions of Taxus chinensis var.Mairei callus.[Method] We compared the efficiencies of callus between different explants and investigated the multiplication conditions of callus and suspended cell culture conditions with the buds,young stems and young leaves from T.chinensis var as the explants.[Results] The effect was the best with the bud as the explants; the best way for sterilizing the explants of T.chinensis var mairei was:streptomycin detergent for 2 h + suds for 3 h + 75% alcohol disinfection for 30 s + 10% sodium hypochlorite solution for 25 min + 1‰ mercury chloride for 10 min; the optimum formula of callus subculture was:B5 + 4.0 mg/L NAA + 0.5 mg/L 2,4-D + 0.2 mg/L GA + 0.5 mg/L 6-BA + 2 g/L AC.[Conclusion] This research built the high efficient regeneration system of T.chinensis var.
文摘Byrsonima intermedia A. Juss. is a species from the Brazilian Cerrado that produces edible fruits and, in common with other species from the Byrsonima genus, has pharmacological potential. Previous attempts to propagate the species through conventional methods showed difficulties. Thus, the purpose of this work was to characterize pro-embryogenic masses of Byrsonima intermedia callus, aiming for their in vitro propagation through somatic embryogenesis. Leaf segments from in vitro germinated seedlings were employed as explants for callus production. The calli were then subcultured and exposed to dyes to fulfill their embryogenic potential. Digitalizations of the cytological preparations were made in order to measure the area that was stained by both Aceto-Carmine and Evans-Blue, using image tool software. Somatic embryos were induced after treatments with l-naphthaleneacetic acid (NAA). The percentages of double-colored areas (by Aceto-Carmine and Evans-Blue) were calculated and the data were analyzed by using the Skott-Knott test (P ≤ 0.05) and, the embryogenic callus, as well as the formation of somatic embryos were analyzed by using the Krsuskal-Wallis rank test (P ≤0.05). The results show that double coloration is effective at identifying cells showing embryogenic potential. Early callus subculture phases show a larger percentage ofembryogenic area (83%) Somatic embryos were induced by using high auxin level.
