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苹果MxIrt1基因的克隆与原核表达
引用本文:王忆,戚金亮,许雪峰,李天忠,孔瑾,韩振海.苹果MxIrt1基因的克隆与原核表达[J].园艺学报,2007,34(4):999-1002.
作者姓名:王忆  戚金亮  许雪峰  李天忠  孔瑾  韩振海
作者单位:(中国农业大学农学与生物技术学院, 北京市果树逆境生理与分子生物学实验室, 北京100094)
基金项目:国家自然科学基金;国家转基因植物专项项目
摘    要:根据植物IRT(Iron Regulated Transporter)家族的功能保守区设计引物,通过RACE法从缺铁胁迫处理的小金海棠根系cDNA文库中克隆得到了Fe2+转运蛋白基因cDNA全长,将其命名为MxIrt1(Malus xiaojinensis Iron regulated transporter 1)。将MxIrt1 cDNA片段与pET30a构建原核表达载体pEIrt,转化大肠杆菌BL21。SDS-PAGE电泳检测结果表明,以30℃、0.5mmol·L-1 IPTG诱导该基因表达效果最好,诱导产物为一个40kD的蛋白。为进一步纯化和鉴定目的蛋白提供了试验基础。

关 键 词:苹果  小金海棠  Fe2+转运蛋白  基因克隆  原核表达  
文章编号:0513-353X(2007)04-0999-04
收稿时间:2006-11-15
修稿时间:2006-11-152007-03-22

Cloning and Prokaryotic Expression of Apple MxIrt1 Gene
WANG Yi,QI Jin-liang,XU Xue-feng,LI Tian-zhong,KONG Jin,HAN Zhen-hai.Cloning and Prokaryotic Expression of Apple MxIrt1 Gene[J].Acta Horticulturae Sinica,2007,34(4):999-1002.
Authors:WANG Yi  QI Jin-liang  XU Xue-feng  LI Tian-zhong  KONG Jin  HAN Zhen-hai
Institution:( Fruit Stress Physiology and Molecular Biology Laboratory of Fruit Tree, College of Agriculture and Biotechnology, China Agricultural University, Beijing 100094, China)
Abstract:A Full length cDNA of MxIrt1 gene from the iron-stressed root cDNA library of Malus xiaojinensis Chent et Jiang was cloned using the RACE method with primers designed based on the conserved domain sequences of plant IRT gene families. The recombinant prokaryotic expression vector pEIrt was constructed using vector pET30a. Restriction endonuclease analysis, PCR amplifying and sequencing confirmed that the construction was correct and had no base mutant. The prokaryotic expression analysis was carried out through transformation of E.coli (BL21). The SDS-PAGE electrophoresis analysis showed that the best expression was induced by 30℃ and 0.5 mmol·L-1 IPTG, under which a 40 kD recombinant protein was produced. These results will provide a foundation for further purifying and identifying objective protein
Keywords:Apple  Malus xiaojinensis  Fe2 -transporter  Gene cloning  Prokaryotic expression
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