[1]廖文林,栾鹤翔,高乐,等.大豆翻译延伸因子GmEF1A干扰载体的构建及大豆遗传转化[J].大豆科学,2016,35(06):902-910.[doi:10.11861/j.issn.1000-9841.2016.06.0902]
 LIAO Wen-lin,LUAN He-xiang,GAO Le,et al.Interference Vector Construction of Soybean Translation Elongation Factor GmeEF1A and Soybean Transformation[J].Soybean Science,2016,35(06):902-910.[doi:10.11861/j.issn.1000-9841.2016.06.0902]
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大豆翻译延伸因子GmEF1A干扰载体的构建及大豆遗传转化

《大豆科学》[ISSN:1000-9841/CN:23-1227/S] 卷: 第35卷 期数: 2016年06期 页码: 902-910 栏目: 出版日期: 2016-11-20
Title:
Interference Vector Construction of Soybean Translation Elongation Factor GmeEF1A and Soybean Transformation
作者:
廖文林栾鹤翔高乐丁雪妮宋英培殷金龙牛浩鹏智海剑
(南京农业大学 国家大豆改良中心/作物遗传与种质创新国家重点实验室,江苏 南京 210095)
Author(s):
LIAO Wen-lin LUAN He-xiang GAO Le DING Xue-ni SONG Ying-peiYIN Jin-longNIU Hao-peng ZHI Hai-jian
(National Center for Soybean Improvement of Nanjing Agricultural University/National Key Laboratory for Crop Genetics and Germplasm Enhancement, Nanjing 210095, China)
关键词:
大豆花叶病毒GmeEF1A基因RNAiGATEWAY技术农杆菌介导大豆遗传转化
Keywords:
Soybean mosaic virus GmeEF1A-gene RNAi GATEWAY technology Agrobacterium-mediated soybean transformation
DOI:
10.11861/j.issn.1000-9841.2016.06.0902
文献标志码:
A
摘要:
研究发现GmeEF1A与大豆花叶病毒的P3蛋白存在互作关系,并且参与SMV在大豆体内的繁殖。通过大豆GmeEF1A基因5个拷贝的核苷酸和氨基酸序列比对,确定其保守区间,克隆得到180 bp的干扰片段GmeEF1Ai。利用GATEWAY技术构建RNA干扰(RNA interference,RNAi)表达载体pB7GWIWG2(II)-eEF1Ai,并通过农杆菌介导的子叶节转化法导入到受体大豆品种天隆1号中。测序结果显示重组质粒中插入的干扰片段GmeEF1Ai与目标序列完全符合,通过PCR和酶切验证表明GmeEF1Ai是以反向重复形式插入到表达载体中。经转化获得组培苗8株,PCR、除草剂涂抹和PAT/bar试纸条多重检测确认7株为阳性。绝对荧光定量结果显示,阳性苗中4株为单拷贝。GmeEF1A基因表达量分析结果显示GmeEF1Ai载体对GmeEF1A的5个拷贝基因有不同程度的阻抑。这不仅为验证GmeEF1A基因在大豆受SMV侵染时的功能提供试验材料,也为大豆抗病育种提供新的种质。
Abstract:
Previous research indicated the interaction between GmeEF1A and P3 protein of soybean mosaic virus, and it is related to SMV replication in soybean. In order to determine the conserved interval of soybean GmeEF1A, we made the nucleotide sequence and amino acid sequence alignment from 5 isoforms of GmeEF1A, cloned the 180 bp interference fragment named GmeEF1Ai. The RNAi vector pB7GWIWG2(II)-eEF1Ai was constructed by GATEWAY technology, and transfered into soybean genotype Tianlong 1 through Agrobacteriummediated system.The sequencing result of GmeEF1Ai fragment in vector matched with the expected sequence completely, and the insert direction was conversed identified by PCR amplification and restriction digestion. We obtained eight transgenic seedlings, seven plants of them were positive detected by PCR, herbicide painting and Liberty Link strip. The data of the fluorescence quantitative PCR showed 4 seedlings contained one copy of bar gene. The results of expression levels of GmeEF1A indicated GmeEF1Ai vector could inhibit the expression of 5 isoforms in different extent. The results of this study provided a material to verify the function of GmeEF1A in SMV resistance and new germplasm resource in soybean mosaic virus- resistance breeding.

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备注/Memo

基金项目:转基因生物新品种培育重大专项(2008ZX08004-004);国家自然科学基金(31371646,31571690);国家现代农业产业技术体系(CARS-004);江苏省现代作物生产协同创新中心(JCIC-MCP)。

第一作者简介:廖文林(1991-),男,硕士,主要从事大豆抗病遗传育种研究。E-mail:423806063@qq.com。通讯作者:智海剑(1957-),男,教授,博导,主要从事大豆抗病遗传育种研究。E-mail:zhj@njau.edu.cn。

更新日期/Last Update: 2016-12-08