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作 者:刘子渲[1] 常柳[2] 张付芸[1] 徐婧[1] 尤明山[1] 梁荣奇[1]
机构地区:[1]中国农业大学农学与生物技术学院植物遗传育种系/农业生物技术国家重点实验室/北京市作物遗传改良重点实验室/农业部作物基因组与遗传改良重点实验室,北京100193 [2]山西大学生物工程学院,太原030006
出 处:《中国农学通报》2012年第12期33-38,共6页Chinese Agricultural Science Bulletin
基 金:国家转基因生物新品种培育重大专项(2009ZX08002-017B)
摘 要:为了获得小麦wx-B1a基因的特异RNAi表达载体,以小麦品种‘京花1号’开花12天的籽粒为材料,用天根公司植物总RNA提取试剂盒提取总RNA,以wx-B1a基因(GenBank NO:AB019623)的cDNA序列设计一对特异性引物,利用RT-PCR克隆了wx-B1a基因部分cDNA片段。Blastn结果显示,它与GenBank上报道的Triticum aestivum wx-1 gene(GenBank NO:EU719611.1)同源。通过酶切连接将此片段分别置于拟南芥FAD2的Intron1(GenBank NO:AJ271841)的上、下游,然后将此发夹结构置于小麦HMW-GS 1Dx5启动子的下游,从而构建了小麦wx-B1a基因的特异RNAi表达载体pBAC47p-wx-B1aIR。从而为下一步转化高产强筋小麦品种培育优质面条专用小麦奠定基础。In order to obtain wheat wx-Bla gene-specific RNAi expression vector, the total RNA was isolated from wheat grain of 12-day post anthering, a pair of special primers was designed according to the wx-Bla gene (GenBank No. AB019623), wx-Bla partial cDNA sequences (461 bp) was amplified by RT-PCR. The results demonstrated that, the cloned wx-Bla gene sequences were high homology with the reported waxy genes in GenBank previously. Then the fragment ligated to the FAD2 Intronl (Arabidopsis FAD2 Intron) in sense and antisense orientation to produce a hairpin fragment. The hairpin fragment was then inserted downstream of the endosperm specific expression promoter of high moleculer weight glutein gene IDx5. And a RNAi vector was obtained, which was drove by HMW-GS 1Dx5 promoter in pBAC47p. This RNAi vector willbe used to breed good-quality noodle lines with high yield-strong gluten wheat.
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