遗传 ›› 2006, Vol. 28 ›› Issue (2): 212-218.

• 技术与方法 • 上一篇    下一篇

一种通用高效的复杂载体构建的新方法

陆云华1;2 ;马立新1; 蒋思婧1   

  1. 1.湖北大学生命科学院分子微生物与基因工程实验室,武汉430062;2.宜春学院生物工程系,江西宜春336000
  • 收稿日期:2005-03-11 修回日期:2005-05-06 出版日期:2006-02-10 发布日期:2006-02-10
  • 通讯作者:

    马立新

A Universal High-throughput Novel Method of Constructing the Vectors

LU Yun-Hua1,2 ,MA Li-Xin1,Jiang Si-Jing1   

  1. 1.Laboratory of  Molecular Microbiology &Gene Engineering, College of Life Science, Hubei University ,Wuhan 430062,China 2.Biotechnology Department of Yichun University, YichunJiangxi Province 33600,China
  • Received:2005-03-11 Revised:2005-05-06 Online:2006-02-10 Published:2006-02-10
  • Contact: MA Li-Xin

摘要:

文章报道了一种简便、通用、高效的复杂载体构建方法。此法是在PCR引物设计时,在目的片段5′端加上随机设计的接头,利用PCR克隆目的片段,再用T4 DNA聚合酶3′→5′外切酶活性处理PCR克隆目的片段,产生多个首尾相匹配的粘性末端,进行多片段定向连接、转化、重组子鉴定。以7片段拼接的水稻单交换质体定点整合表达载体pRSMGA的构建为例,应用上述方法构建只需做两次连接、转化,且其重组、转化效率高。数10次实验证明:这是一种简便、通用、高效的复杂构建载体的方法,该法至今尚未见报道。
 
 
 

关键词: 复杂载体构建, 新方法, T4DNA聚合酶, 水稻

Abstract: In this paper, a simple universal high-throughput method of constructing the vectors was developed. It could add proper adapter when the PCR primers were designed, and the purpose fragments were cloned by PCR, and the various complementary sticky ends were created by T4 DNA polymerase’s 3′-exodeoxyribonuclease activity. If all these fragments were put together with DNA ligase, they would recombinate in an orientation. If they had been transformated, the tansformants would be identified. Let’s take the Oryza sativa single-cross homologous recombination chloroplast expression vector pRSMGA which was constructed with seven fragments as an example, if the vector pRSMGA was constructed in using the method what had mentioned, only twice recombination and transformation would be done. Scores of experiments had proved that it is a simple universal high-throughput novel method to construct the complicated vectors, which has not appeared in the periodical.

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