摘要
将0.5%纤维素酶Rs+0.1%果胶酶Y-23酶溶液振荡处理3h,可得到最高的细胞分裂率,但原生质体分离数量较低。0.5%纤维素酶R-10+0.05%离析酶R-10+0.05%果胶酶Y-23酶溶液,25℃下处理14h,原生质体分离数量及细胞分裂率均较高。1/2MS培养基添加NAA3mg/L+BA0.5mg/L+2,4-D 0.1mg/L的液体培养基有利于细胞团形成及愈伤组织生长。本试验获得了完整的再生植株,芽分化率达20%左右。
Through the treatment of application of 0.5% cellulase Rs+0.1% pectolyase Y-23 by shaking for 3h, the highest cell division efficiency was obtained, but the number of protoplast isolation was relatively low. Also, through the treatments using enzyme mixture of 0.5% cellulase R-10+0.05% macerozyme R-10+0.005% pectolyase Y-23 incubated at 25℃: for 14h, more protoplasts were isolated and a high efficiency of cell division was gained. The liquid medium of 1 / 2 MS containing 3 mg/ L NAA, 0.5 mg/ L BA and 0.1 mg/ L 2,4-D was favourable to the formation of cellular aggreate and the callus growth. Complete plantlets regenerated were obtained, and the bud differentiation rate can reach 20% or so in this experiment.
出处
《西北农业大学学报》
CSCD
1993年第1期100-102,共3页
Journal of Northwest Sci-Tech University of Agriculture and Forestry(Natural Science Edition)
关键词
甘蓝
子叶
原生质体培养
植株再生
Brassica oleracea
Cotyledons
Protoplast culture
liquid media
phytohormones / plantlet regeneration
