| Literature DB >> 33654750 |
Claudia Cattoglio1,2,3,4, Iryna Pustova1,2,3,4, Xavier Darzacq1,2,3, Robert Tjian1,2,3,4, Anders S Hansen1,2,3,4.
Abstract
Protein-protein interactions constitute the molecular foundations of virtually all biological processes. Co-immunoprecipitation (CoIP) experiments are probably the most widely used method to probe both heterotypic and homotypic protein-protein interactions. Recent advances in super-resolution microscopy have revealed that several nuclear proteins such as transcription factors are spatially distributed into local high-concentration clusters in mammalian cells, suggesting that many nuclear proteins self-interact. These observations have further underscored the need for orthogonal biochemical approaches for testing if self-association occurs, and if so, what the mechanisms are. Here, we describe a CoIP protocol specifically optimized to test self-association of endogenously tagged nuclear proteins (self-CoIP), and to evaluate the role of nucleic acids in such self-interaction. This protocol has proven reliable and robust in our hands, and it can be used to test both homotypic and heterotypic (CoIP) protein-protein interactions.Entities:
Keywords: Cas9-mediated endogenous tagging; Co-immunoprecipitation; CoIP; IP; Immunoprecipitation; Self-interaction
Year: 2020 PMID: 33654750 PMCID: PMC7842838 DOI: 10.21769/BioProtoc.3526
Source DB: PubMed Journal: Bio Protoc ISSN: 2331-8325