2008
DOI: 10.1089/adt.2008.137
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Development of the Predictor hERG Fluorescence Polarization Assay Using a Membrane Protein Enrichment Approach

Abstract: The life-threatening consequences of acquired, or drug-induced, long QT syndrome due to block of the human ether-a-go-go-related gene (hERG) channel are well appreciated and have been the cause of several drugs being removed from the market in recent years because of patient death. In the last decade, the propensity for block of the hERG channel by a diverse and expanding set of compounds has led to the requirement that all new drugs be tested for hERG channel block in a functional patch-clamp assay. Because o… Show more

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Cited by 46 publications
(50 citation statements)
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“…Our ability to predict which small molecules will block hERG is poor and therefore all compounds under consideration for drug development are tested in a hERG activity assay. Several assays exist: cell-based functional assays, such as thallium and/or rubidium flux, nonfunctional assays, such as ligand binding and/or fluorescence polarization, and electrophysiology (22,23,31,32). The gold standard is electrophysiology, but it can be slow and expensive when the need exists for evaluating many compounds.…”
Section: Significancementioning
confidence: 99%
“…Our ability to predict which small molecules will block hERG is poor and therefore all compounds under consideration for drug development are tested in a hERG activity assay. Several assays exist: cell-based functional assays, such as thallium and/or rubidium flux, nonfunctional assays, such as ligand binding and/or fluorescence polarization, and electrophysiology (22,23,31,32). The gold standard is electrophysiology, but it can be slow and expensive when the need exists for evaluating many compounds.…”
Section: Significancementioning
confidence: 99%
“…For example, a homogeneous, fluorescence polarization-based assay to characterize the affinity of small molecules for the hERG channel was recently reported [40]. This assay has demonstrated tight correlation with data obtained from patch-clamp assays.…”
Section: Non-electrophysiological Approaches For Determining Herg Chamentioning
confidence: 97%
“…Fluorescence intensity (Excitation at 530 nm, Emission at 590 nm) was measured using a multi-mode microplate reader Synergy Neo (Biotek, Winooski, VT, USA). E-4031 was used as the reference positive standard (IC 50 = 10-90 nM) [20].…”
Section: Cyp Inhibition Assaymentioning
confidence: 99%