| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 4503279 | Acta Agronomica Sinica | 2010 | 6 Pages |
Late embriogenesis abundant (LEA) protein is one of the hot topics in plant stress physiology. In this study, an RNAi expression vector harboring MsLEA3-1 gene fragment from alfalfa (Medicago sativa L.) was constructed. Two pairs of specific primers with different enzyme sites were designed based on the sequence of MsLEA3-1 (GenBank accession number EU665182). With the template of PMD-LEA plasmid constructed, positive-sense strand and antisense strand were obtained, which were separately inserted into the expression vector pART27. A hairpin structure in the RNAi vector pART-F-R was confirmed by the digestion of restriction enzymes. pART-F-R was transformed into tobacco via Agrobacterium-mediated transformation system, and 16 transgenic plants were obtained after PCR validation.
摘 要根据紫花苜蓿LEA蛋白MsLEA3-1基因(GenBank登录号为EU665182)序列, 设计两对含有酶切位点的特异性引物LEAf1/ LEAf2和LEAr1/LEAr2, 以构建好的PMD-LEA质粒为模板, 分别合成用于构建干扰载体的正反义片段pMD-F和pMD-R, 将正反义片段分别插入表达载体pART27的相应位置, 构建成含有发夹结构的RNAi载体pART-F-R, 经过Not I酶切鉴定, 证明载体构建成功。通过农杆菌介导的方法, 以干扰表达载体pART-F-R转化烟草, 经过PCR检测, 得到16株阳性转基因植株, 为MsLEA3-1基因的功能研究奠定基础。
