作物学报 ›› 2011, Vol. 37 ›› Issue (07): 1205-1211.doi: 10.3724/SP.J.1006.2011.01205
张庆林1,赵艳2,**,李晓薇1,翟莹1,张艳1,王英1,李景文1,*,王庆钰1,*
ZHANG Qing-Lin1,ZHAO Yan2,**,LI Xiao-Wei1,ZHAI Ying1,ZHANG Yan1,WANG Ying1,LI Jing-Wen1,*,WANG Qing-Yu1,*
摘要: 以吉豆2号基因组为模板,通过TAIL PCR方法,扩增得到大豆硬脂酸-ACP脱饱和酶基因启动子片段SACPD-Cp。PLACE在线启动子预测分析表明, 该序列中含有多种典型的种子特异性表达序列元件。将SACPD-Cp片段取代pCAMBIA1301质粒中的CaMV35S启动子,构建表达载体pCAM-SACPD-Cp,通过农杆菌介导法在大豆组织中进行瞬时表达,GUS组织化学染色和荧光定量研究其表达特性。结果表明, SACPD-Cp驱动GUS基因在种子中的表达活性是CaMV35S启动子的93.01%;SACPD-Cp启动子与现已知启动子无同源性,仅在大豆种子中检测到GUS活性,而在根、茎和叶组织中均未检测到GUS活性,证实 SACPD-Cp是一个新的种子特异性启动子。
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