Journal
JOURNAL OF BIOMOLECULAR SCREENING
Volume 12, Issue 5, Pages 694-704Publisher
SAGE PUBLICATIONS INC
DOI: 10.1177/1087057107301497
Keywords
Photina (R); photoprotein; flash luminescence; HTS; cell-based assays; GPCR
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The present work describes the engineering and characterization of a new Ca2+ -activated photoprotein (Photina (R)) and its use in mammalian cell lines for implementation of flash luminescence cell-based assays for high-throughput screening (HTS). When used to measure the activation of 2 G protein-coupled receptors (GPCRs), targeting Photina((R)) to the mitochondria increased the signal strength as compared to the normal cytoplasmic expression of Photina((R)) The mitochondrial-targeted Photina((R)) also produced a higher signal-to-noise ratio than conventional calcium dyes and a consistently stronger signal than aequorin when tested under equivalent conditions. MitoPhotina((R)) provided strong and reliable results when used to measure the activity of purinergic receptors endogenously expressed in the Chinese Hamster Ovary cells and heterologously expressed GPCRs in response to their cognate ligands. Several different types of flash luminescence plate readers (FLIPR (R), FLIPR (R). CyBi (R)-Lumax flash HT, Lumilux((R)), Lumibox) in different plate formats (96, 384, 1536 wells) were used to validate the use of Photina((R)) in HTS. The cell number had to be adjusted to correspond to the qualities of the different readers, but once so adjusted, it provided equivalent results on each device. The results obtained show robust and reproducible light signals that offer new possibilities for application of photoproteins to the -,eneration of cell-based assays for HTS.
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