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作 者:郝璞 薄高峰 刘璐[1] 白鹤鸣 吴凤霞 周星雨 杨海峰[1] Hao Pu;Bo Gaofeng;Liu Lu;Bai Heming;Wu Fengxia;Zhou Xingyu;Yang Haifeng(Forestry College of Inner Mongolia Agricultural University,Hohhot 010018,China)
机构地区:[1]内蒙古农业大学林学院,内蒙古呼和浩特010018
出 处:《山东农业科学》2021年第11期1-7,共7页Shandong Agricultural Sciences
基 金:国家自然科学基金项目(31660216);国家科技重大专项课题(2018ZX08020002-005-005);内蒙古自治区应用技术研究与开发项目“内蒙古地区多功能树种选育及扩繁关键技术研究与示范”(2019GG004);优质沙生灌木种质资源开发、利用关键技术项目(2021GG0075)。
摘 要:TAC(tiller angle control)基因作为IGT [G?L(A/T)IGT]保守家族的一员,与植物体内各类激素相互作用,共同参与分枝角度的调控。为探究TAC基因的分子结构功能及其调节功能,利用CRISPR/Cas9基因编辑系统,以INRA717-1B4杂交杨为试验材料构建pDE-CAS9-NPTⅡ表达载体,通过农杆菌介导法侵染叶片进行遗传转化获得阳性植株,并通过测序检测基因编辑效率。最终获得基因编辑转基因株系12株,其中实现基因突变的2株,编辑效率为16.7%。本试验为CRISPR/Cas9系统在杨树TAC基因功能的验证提供了借鉴,为进一步在木本植物中的应用研究提供了技术支持。As a member of the IGT(G?L(A/T)IGT) family, TAC(tiller angle control) gene interacts with various hormones in the plant and is involved in the regulation of branching angle. To explore the molecular structure function and regulatory function of TAC gene, the pDE-CAS9-NPTⅡ expression vector was successfully constructed using the CRISPR/Cas9 gene-editing system with the INRA717-1 B4 hybrid poplars as experimental materials. The leaves were infected by Agrobacterium-mediated method for genetic transformation, and positive plants were obtained. The gene editing efficiency was tested by sequencing. Finally, 12 transgenic lines were obtained, of which, gene mutation was realized in 2 lines, and the editing efficiency was 16.7%. This study could provide a reference for verifying the function of TAC gene in hybrid poplars with CRISPR/Cas9 system, and provide technical support for further application research in woody plants.
关 键 词:INRA717-1B4杂交杨 CRISPR/Cas9系统 TAC基因 载体构建 编辑效率
分 类 号:S792.119[农业科学—林木遗传育种] Q782[农业科学—林学]
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