A novel, easy and rapid method for constructing yeast two-hybrid vectors using In-Fusion technology

Author:

Yu Deshui12,Liao Libing23,Zhang Ju12,Zhang Yi124,Xu Kedong12,Liu Kun12,Li Xiaoli12,Tan Guangxuan12,Chen Ran123,Wang Yulu123,Liu Xia123,Zhang Xuan123,Han Xiaomeng123,Wei Zhangkun123,Li Chengwei125

Affiliation:

1. Key Laboratory of Plant Genetics & Molecular Breeding, Zhoukou Normal University, Zhoukou, 466001, PR China

2. Henan Key Laboratory of Crop Molecular Breeding & Biorector, Zhoukou, 466001, PR China

3. College of Life Science & Agronomy, Zhoukou Normal University, Zhoukou, 466001, PR China

4. College of Agronomy, Henan Agricultural University, Zhengzhou, 450002, PR China

5. Henan Engineering Research Center of Crop Genome Editing, Henan Institute of Science & Technology, Xinxiang, 453003, PR China

Abstract

Yeast two-hybrid systems are powerful tools for analyzing interactions between proteins. Vector construction is an essential step in yeast two-hybrid experiments, which require bait and prey plasmids. In this study, we modified the multiple cloning site sequence of the yeast plasmid pGADT7 by site-directed mutagenesis PCR to generate the pGADT7-In vector, which resulted in an easy and rapid method for constructing yeast two-hybrid vectors using the In-Fusion cloning technique. This method has three key advantages: only one pair of primers and one round of PCR are needed to generate bait and prey plasmids for each gene, it is restriction endonuclease- and ligase-independent, and it is fast and easily performed.

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology

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