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通过转重复结构的ACC氧化酶基因延长香石竹的瓶插期
引用本文:余义勋,包满珠. 通过转重复结构的ACC氧化酶基因延长香石竹的瓶插期[J]. 植物生理与分子生物学学报, 2004, 30(5): 541-545
作者姓名:余义勋  包满珠
作者单位:华中农业大学园艺林学学院,园艺植物生物学教育部重点实验室,武汉,430070
摘    要:以香石竹叶片为外植体,用农杆菌(Agrobacteriumtumefaciens)介导法,在选择分化培养基中培养后,将香石竹重复结构的ACC氧化酶(ACO)基因核DNA导入香石竹‘Maber品种.经Southera杂交检测,证明外源基因已整合到香石竹基因组,共获得3株转化植株.转基因植株在隔离条件下栽培时正常开花,转基因T257株系切花衰老过程中乙烯释放量较对照低95%,没有乙烯跃变峰出现.在25℃条件下比较瓶插期,有2个转化株系瓶插期显著延长,最长比对照长了5 d以上.

关 键 词:香石竹  ACC氧化酶(ACO)基因  转化  瓶插期  乙烯  基因沉默
修稿时间:2003-12-24

Prolonging the Vase Life of Carnation 'Mabel' Through Integrating Repeated ACC Oxidase Genes into Its Genome
YU Yi-Xun,BAO Man-Zhu. Prolonging the Vase Life of Carnation 'Mabel' Through Integrating Repeated ACC Oxidase Genes into Its Genome[J]. Journal Of Plant Physiology and Molecular Biology, 2004, 30(5): 541-545
Authors:YU Yi-Xun  BAO Man-Zhu
Affiliation:Key Laboratory of Horticultural Plant Biology, Ministry of Education, College of Horticulture and Forestry Sciences, Huazhong Agricultural University, Wuhan 430070, China.
Abstract:Carnation (Dianthus caryophyllus L.) is one of the most important cut flowers. The cultivar "Mabel" of carnation was transformed with direct repeat gene of ACC oxidase, the key enzyme in ethylene synthesis, driven by the CaMV35S promoter mediated by Agrobacterium tumefacien. Hygromycin phosphotransferase (HPT) gene was used as selection marker. Leaf explants were pre-cultured on shoot-inducing medium for 2 d, then immersed in Agrobacterium suspension for 8-12 min. Co-cultivation was carried out on the medium (MS+BA 1.0 mg/L+NAA 0.3 mg/L +Acetosyringone 100 micromol/L, pH 5.8-6.0) for 3 d. After that transformants were obtained by transferring explants to selection medium supplemented with 5 mg/L hygromycin (Hyg) and 400 mg/L cefotaxime (Cef). Southern blotting detection showed that a foreign gene was integrated into the carnation genome and 3 transgenic lines (T257, T299 and T273 line) obtained. Addition of acetosyringone and the time of co-culture were the main factors that influenced transformation frequency. After being transplanted to soil, transgenic plants were grew normally in greenhouse. Ethylene production of cut flower of transgenic T257 line was 95% lower than that of the control, and that of T299 line was reduced by 90% than that of the control, while that of transgenic T273 line has no of significantly different from control. Vase life of transgenic T257 line was 5 d longer than that of the control line at 25 degrees C.
Keywords:carnation (Dianthus caryophyllus L.)  ACC oxidase(ACO)gene  transformation  vase life  ethylene  gene silencing
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