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机构地区:[1]中国科学院植物研究所,光合作用与环境分子生理学重点实验室,北京100093 [2]山西师范大学生命科学学院,临汾041004
出 处:《植物学通报》2008年第3期322-331,共10页Chinese Bulletin of Botany
基 金:国家自然科学基金(No.30670185)
摘 要:以成熟胚愈伤组织为材料的农杆菌介导水稻转化法虽已建立,但转化频率仍有待提高。本文以粳稻(Oryzasativa)品种(中花10号和中花11号)的成熟胚诱导的愈伤组织为受体材料,对组织培养体系及影响遗传转化的因素进行优化,建立了一套改进的农杆菌介导的水稻高效遗传转化系统。农杆菌菌株为EHA105,质粒载体是pUN1301/OsRAA1,其中含有标记基因GUS和筛选基因HPT。愈伤组织诱导培养基为NBD2(NB+2mg·L^(-1)2,4-D),继代培养基为NBD0.5,预分化与分化培养基为RE1(MS+1mg·L^(-1)6-BA+0.25mg·L^(-1)NAA+0.5mg·L^(-1)KT+0.2mg·L^(-1)ZT)和RE2(MS+1mg·L^(-1)6-BA+0.5mg·L^(-1)NAA+0.5mg·L^(-1)KT+0.2mg·L^(-1)ZT)。另外,还分析了影响T-DNA转移的多种因素,如外植体种类、愈伤组织预培养基和愈伤组织继代次数等。采用优化的转化程序,水稻愈伤组织转化率和植株转化率可达70%以上。Rice has been transformed via Agrobacterium transfection with use of mature embryo-derived calli, but the transformation efficiency has remained relatively low in general. In this study, we optimized different factors affecting transformation and established a highly efficient transformatiom system mediated by Agrobacterium using mature embryo-derived calli from two japonica cultivars (Zhonghua 10, 11 ). The transformation was performed with A. tumefaciens strain EHA105 harboring the plasmid pUN1301/OsRAA1, GUS used as the reporter gene and HPT as the selectable marker gene. First, we established a high-frequency regeneration system for rice, defined NBD2 (NB+2 mg.L^-1 2,4-D) as callus induction medium, NBD0.5 as subculture medium, and RE1 (MS+1 mg.L^-1 6-BA+0.25 mg.L^-1 NAA+0.5 mg.L^-1 KT+0.2 mg.L^-1 ZT) and RE2 (MS+1 mg.L^-1 6-BA+0.5 mg.L^-1NAA+0.5 mg.L^-1 KT+0.2 mg.L^-1 ZT) as regeneration medium. Second, factors such as the selection of explants, the pre-culture medium and the subculture times were shows to affect the efficiency of T-DNA delivery. The transformation efficiency using the optimized method was increased to 70%, which was measured either by counting the number of hygromycin-resistant calli or the number of transgenic plants.
关 键 词:农杆菌介导的遗传转化 成熟胚诱导的愈伤组织 水稻
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