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. 2008 Feb 6;9:68. doi: 10.1186/1471-2164-9-68

Figure 1.

Figure 1

Cell array based PPI screens in different cell lines. 1a: Transfection efficiency and specific protein-protein interaction in different cell lines is demonstrated using the Gal4-pZsGreen reporter and plasmids coding for the known interacting p53 (pBD-p53) and SV40-T (pAD-SV40T) hybrid proteins (boxed, line B). As negative control (line A) Gal4-pZsGreen reporter was co-transfected with the non-interacting proteins p53 (pBD-p53) and TRAF (pAD-TRAF). The pBD-NF-κB control plasmid expressing the GAL4 DNA-binding domain fused to the transcription activation domain of NF-κB is used as a positive control to monitor transfection efficiency and reporter performance (line C). A construct expressing EGFP under control of a CMV promoter (line D) is typically printed as a frame at the periphery of the arrays in order to locate the arrayed features. Fig. 1a shows example images of different adherent cell lines transfected using identical microarray slides. 1b: Transfection efficiency as reflected by the level of NF-κB induced reporter expression. Comparable results were obtained for PC-3, HEK293 and HeLa. Data shown are from representative experiments and represent mean fluorescence of 6 features per sample, collected from triplicate spots on two identical slides.