Published: Vol 6, Iss 9, May 5, 2016 DOI: 10.21769/BioProtoc.1800 Views: 16651
Reviewed by: Zhaohui LiuPablo Bolanos-VillegasAnonymous reviewer(s)
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Abstract
Studying protein-protein interaction is crucial to understand the fundamental processes of molecular biology. High-throughput screening, such as immunoprecipitation followed by proteomic analysis, allows for the identification of numerous candidate partners that might interact with a selected protein. However, experimental validation of protein-protein interaction requires conventional cloning and recombinant protein expression/purification, which are complicated and labor-intensive techniques. Here, we demonstrate an efficient experimental pipeline for verifying protein-protein interactions between a bait protein using the example of Odontoglossum ringspot virus (ORSV) capsid protein (CP) and the host CP-binding protein. These candidate CP-binding proteins were identified through high-throughput proteomic and transcriptomic approaches. Using the TOPO cloning strategy, each candidate gene was cloned into an expression vector for the expression of His-tagged recombinant proteins in a single step of an in vitro transcription/translation system. Such expressed His-tagged candidates can be used as prey with the CP bait protein in a co-immunoprecipitation (co-IP) assay to verify their physical interaction. Without the need for traditional protein expression and purification, this pipeline simplifies the validation process and provides a solution for high-throughput protein-protein interaction studies.
Keywords: Protein-protein interactionMaterials and Reagents
Equipment
Procedure
Figure 1. Illustration of the in vitro detection of the protein interaction procedure. A. Genes encoding prey proteins are cloned into the pEXP5-CT/TOPO vector using the TOPO cloning system. B. Expression of C-terminal His-tagged recombinant proteins by cell-free in vitro transcription/translation. C. Co-immunoprecipitation is performed to analyze interaction between the His-tagged prey and GST-tagged bait using a bait-specific antibody. An anti-His antibody was used for prey detection and an anti-GST antibody for examining bait precipitation.
Component | Amount |
Purified DNA (0.05-1 μg) | x μl |
Salt solution | 0.5 μl |
pEXP5-CT/TOPO® vector | 0.5 μl |
H2O | To 3 μl |
Component | Amount |
E. coli slyD- extract | 5 μl |
2.5x IVPS buffer | 5 μl |
50 mM amino acids (without met) | 0.3125 μl |
75 mM methionine | 0.25 μl |
T7 enzyme mix | 0.25 μl |
pEXP5 plasmid DNA | 1 μg |
H2O | To 12.5 μl |
Component | Amount |
2x IVPS feed buffer | 6.25 μl |
50 mM amino acid | 0.3125 μl |
75 mM methionine | 0.25 μl |
H2O | To 12.5 μl |
Recipes
Acknowledgments
This work was supported by grants from the Ministry of Science and Technology, Taiwan (NSC-102-2313-B-002-068-MY3 and NSC-102-2313-B-002-066-B-MY3) to S.-S. Lin and (NSC-99-2313-B-002-043-MY3) to Y.-C. Chang.
References
Article Information
Copyright
© 2016 The Authors; exclusive licensee Bio-protocol LLC.
How to cite
Lin, P., Chang, Y. and Lin, S. (2016). An in vitro Transcription/translation System for Detection of Protein Interaction. Bio-protocol 6(9): e1800. DOI: 10.21769/BioProtoc.1800.
Category
Molecular Biology > Protein > Protein-protein interaction
Plant Science > Plant molecular biology > Protein
Microbiology > Microbe-host interactions > Virus
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