Protein-fragment complementation assay the field of molecular biology , a protein-fragment complementation assay , or PCA, is a method for the identification and quantification of protein–protein interactions . In the PCA, the proteins of interest are each covalently linked to fragments of a third protein . Interaction between the bait and the prey proteins brings the fragments of the reporter protein in close proximity to allow them to form a functional reporter protein whose activity can be measured. This principle can be applied to many different reporter proteins and is also the basis for the yeast two-hybrid system , an archetypical PCA assay.Split protein assays Any protein that can be split into two parts and reconstituted non-covalently to form a functional protein may be used in a PCA. The two fragments however have low affinity for each other and must be brought together by other interacting proteins fused to them. The protein that produces a detectable readout is called "reporter". Usually enzymes which confer resistance to nutrient deprivation or antibiotics, such as dihydrofolate reductase or beta-lactamase respectively, or proteins that give colorimetric or fluorescent signals are used as reporters. When fluorescent proteins are reconstituted the PCA is called Bimolecular fluorescence complementation assay . The following proteins have been used in split protein PCAs:Beta-lactamase Dihydrofolate reductase Focal adhesion kinase Gal4, a yeast transcription factor GFP, e.g. EGFP Horseradish peroxidase Infrared fluorescent protein IFP1.4, an engineered chromophore-binding domain of a bacteriophytochrome from Deinococcus radiodurans LacZ Luciferase, including ReBiL and Gaussia princeps luciferase . Commercial products using luciferase include NanoLuc and NanoBIT. A modification has also been developed for lipid droplet-associated interactions. TEV Ubiquitin
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