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出 处:《武汉大学学报(自然科学版)》1994年第4期89-94,共6页Journal of Wuhan University(Natural Science Edition)
基 金:国家自然科学基金
摘 要:研究了光敏感核不育水稻的悬浮细胞及愈伤组织的低温贮藏方法.实验采用10%DMSO+0.5mol·L-1山梨醇作冰冻保护剂,降温速率采用1.0℃·min-1或0.5℃·min-1,TTC法测试的细胞存活率最高可达85.9%,冻后材料经15d左右即可在暗培养条件下观察恢复生长的情况.30d后把长势良好的愈伤组织块转移至分化培养基中,来源于悬浮细胞团的绿苗分化率为10.0%,愈伤组织的则为66.6%.This paper mainly reported the cryopreservation method of callus and cellsuspensions of HPGMR. Cell line (N5047s)and callus (Nong Keng 58s) were derived fromyoung panicles culture. By preculturing-freezing-liquid nitrogen cryopreserving-rapidthawing, the highest cell viability (TTC test)was 85. 9%.The mixture of cryoprotectant of 10%DMSO plus 0. 5ml0. 5L-1 sorbitol was optimal,and slow freezing with a temperature of 1.0℃· min-1 or 0. 5℃·min-1 was recommended. After 15 days’ dark culture, the recoverygrowth of frozen materials was observed. Then we transfered the callus to differentiation culture medium. The plantlet differentiation rate from cell suspensions was 10. 0%, and thatfrom callus was 66. 6%.
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