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Merck

A real-time fluorometric method for the simultaneous detection of cell death type and rate.

Nature protocols (2016-07-16)
Sasker Grootjans, Behrouz Hassannia, Iris Delrue, Vera Goossens, Bartosz Wiernicki, Yves Dondelinger, Mathieu J M Bertrand, Dmitri V Krysko, Marnik Vuylsteke, Peter Vandenabeele, Tom Vanden Berghe
RESUMEN

Several cell death assays have been developed based on a single biochemical parameter such as caspase activation or plasma membrane permeabilization. Our fluorescent apoptosis/necrosis (FAN) assay directly measures cell death and distinguishes between caspase-dependent apoptosis and caspase-independent necrosis of cells grown in any multiwell plate. Cell death is monitored in standard growth medium as an increase in fluorescence intensity of a cell-impermeable dye (SYTOX Green) after plasma membrane disintegration, whereas apoptosis is detected through caspase-mediated release of a fluorophore from its quencher (DEVD-amc). The assay determines the normalized percentage of dead cells and caspase activation per condition as an end-point measurement or in real time (automated). The protocol can be applied to screen drugs, proteins or siRNAs for interference with cell death while simultaneously detecting cell death modality switching between apoptosis and necrosis. Initial preparation may take up to 5 d, but the typical hands-on time is ∼2 h.

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Sigma-Aldrich
Staurosporine from Streptomyces sp., for molecular biology, ≥95% (HPLC)
Sigma-Aldrich
Anticuerpo anti-Fas (humano, activador), clon CH11, clone CH11, Upstate®, from mouse
Sigma-Aldrich
Necrostatin-1, Necrostatin-1, CAS 4311-88-0, is a cell-permeable, potent, and selective blocker of necroptosis (EC₅₀ = 494 nM in FADD-deficient Jurkat cells treated with TNF-α).