A new Alamar Blue viability assay to rapidly quantify oligodendrocyte death

We developed a rapid fluorometric viability assay for primary cultures of O L precursors (preOLs) or mature OLs that utilized the oxidation/reduction i ndicator dye Alamar Blue (AB). PreOLs had a lower rate of AB reduction than did mature OLs (0.02 +/- 0.01 units/min per cell versus 0.07 +/- 0.01). Th e assay was tested under two conditions toxic to preOLs: oxidative stress i nduced by glutathione depletion or kainate excitotoxicity. When glutathione was depleted by a 24-h exposure to cystine-depleted medium, the EC50 value s for the dependence upon cystine for survival did not differ significantly when determined by AB reduction (2 +/- 2 mu M), by the trypan blue exclusi on method (3 +/- 3 mu M) or by MTT histochemistry (1 +/- 0.4 mu M). Quantif ication of preOL viability with AB was unaffected by the presence of free r adical scavengers (alpha-tocopherol or idebenone) or the antioxidant enzyme s Cu,Zn-superoxide dismutase and catalase. There was no difference in preOL viability as determined by AB or MTT after a 24-h exposure to kainate at c oncentrations up to 1 mM. AR offers a rapid objective measure of OL viabili ty in primary culture and is a valid means to quantify OL death. (C) 1999 E lsevier Science B.V. All rights reserved.