摘要
[目的]研究外源蛋白定位马铃薯淀粉粒表达载体的构建,为解决从植物中分离外源蛋白成本高及表达量低的产业化核心问题提供参考。[方法]利用RT-PCR、巢式PCR等分子生物学技术,构建使外源蛋白定位表达于马铃薯淀粉粒的植物表达载体。[结果]克隆获得GBSSI定位表达于马铃薯淀粉粒的编码序列(GC20);通过连接、转化和酶切鉴定筛选出马铃薯块茎专一性启动子GBSSI启动子驱动GC20的植物表达载体。[结论]该研究结果为进一步在马铃薯淀粉粒上筛选外源蛋白奠定了基础。
[ Objective ] The research aimed to study construction of expression vector of foreign protein locating potato starch grain, and provide some reference for solving industrialized core problem of high cost and low expression level of foreign protein. [ Method] By using molecu- lar biological techniques of RT-PCR and Nest type PCR, plant expression vector for the foreign protein locating the potato starch grains was constructed. [ Resuh] Coding sequence (GC20) of potato starch grain which located and expressed by GBSSI was cloned. Plant expression vector was screened out through connection, transformation and enzyme digestion identification. [ Conclusion ] This result of study laid a foundation for further sereening the foreign protein on the potato starch grains.
出处
《安徽农业科学》
CAS
北大核心
2009年第31期15167-15168,共2页
Journal of Anhui Agricultural Sciences
基金
国家自然科学基金项目(30160010)