| Literature DB >> 28032891 |
Sofie De Munter1, Janina Görnemann1, Rita Derua2,3, Bart Lesage1, Junbin Qian1, Ewald Heroes1, Etienne Waelkens2,3, Aleyde Van Eynde1, Monique Beullens1, Mathieu Bollen1.
Abstract
The biotin identification (BioID) protocol uses a mutant of the biotin ligase BirA (BirA*) fused to a protein-of-interest to biotinylate proximate proteins in intact cells. Here, we show that two inactive halves of BirA* separately fused to a catalytic and regulatory subunit of protein phosphatase PP1 reconstitute a functional BirA* enzyme upon heterodimerization of the phosphatase subunits. We also demonstrate that this BirA* fragment complementation approach, termed split-BioID, can be used to screen for substrates and other protein interactors of PP1 holoenzymes. Split-BioID is a novel and versatile tool for the identification of (transient) interactors of protein dimers.Entities:
Keywords: biotinylation; phosphatase-substrate mapping; protein-ligand screening; proximity labeling; reporter-fragment complementation
Mesh:
Year: 2017 PMID: 28032891 DOI: 10.1002/1873-3468.12548
Source DB: PubMed Journal: FEBS Lett ISSN: 0014-5793 Impact factor: 4.124