Fig. 2.

Flow cytometry analysis of chromosomally integrated yEGFP reporter fluorescence in the Y187 strain. Y187-yEGFP cells were transformed with several protein pairs and the colonies grown on SD-L-T plates were suspended in PBS buffer and used for GFP fluorescence analysis by flow cytometry. The percentage of positive GFP cells triggered by the P53/T and BD/PCL1 constructs were shown by using the Lam/T pair as the negative control.