Detection of Protein-Protein Interactions Using Nonimmune IgG and Bira-Mediated Biotinylation | Zendy

Cai Huang | Zendy; Ken Jacobson | Zendy

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Detection of Protein-Protein Interactions Using Nonimmune IgG and Bira-Mediated Biotinylation

Author(s) -

Cai Huang,

Ken Jacobson

Publication year - 2010

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/000113550

Subject(s) - biotinylation , immunoprecipitation , streptavidin , fusion protein , western blot , protein subcellular localization prediction , protein g , sepharose , antibody , protein a , protein a/g , protein–protein interaction , microbiology and biotechnology , protein detection , biology , tandem affinity purification , blot , biotin , biochemistry , affinity chromatography , gene , recombinant dna , immunology , enzyme , materials science , nanotechnology

Detection of protein-protein interactions in cells is crucial for understanding the biological functions of proteins, including their roles in signal transduction. However, current methods require specific antibodies both for immunoprecipitation and detection, making them expensive and sometimes unreliable. Here we describe protocols for protein-protein interaction assays that use nonimmune IgG-conjugated Sepharose to precipitate the IgG binding domain (ZZ) fused to the bait protein; the interaction partner is fused to Avitag and biotinylated by BirA so that it can be detected by a one-step blot with Dylight 680 streptavidin to detect the Avitag fusion protein. Since this method does not require specific antibodies and is inexpensive, sensitive, and reliable, it should be useful for detecting protein-protein interactions in cells.

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