E solution (C ). Fluo3-AM green fluorescence was used for evaluation of the cytosolic calcium levels. Each bar represents the mean value from three determinations with the standard deviation (SD). Data (mean 6 SD) with asterisk significantly differ (*p,0.05; **p,0.01) between treatments. doi:10.1371/journal.pone.0060462.gpeptides would induce membrane lipid asymmetry, membrane integrity disruption and enhancement of membrane permeability (as indicated by increased cell surface PS exposure and PI/EthD-1 uptake). Moreover, although temporin-1CEa of 20 mM was excluded from cancer cells, the peptides are still able to trigger intracellular events, including intracellular ROS and calcium ion elevation, transmembrane potential depolarization and loss of mitochondrial membrane potential. The calcium-related mechanisms have been identified to be involved in cell death induced by some certain antimicrobial peptide [29]. In our present study, the increased intracellular calcium concentration induced by 20 mM temporin-1CEa exposure was partlyly mediated by the endogenous calcium released from intracellular stores and have pivotal roles in temporin-1CEa-induced breast cancer cells death, although the detailed intracellular signaling pathway awaits further investigation. When cancer cells were exposed to temporin-1CEa of higher concentrations, temporin-1CEa might induce membrane pore, or directly disrupt cell membranes to lysis. This membrane-disrupting effect resulted in PS exposure, membrane permeablization and even the release of cytoplasmic contents out of the cell, which ultimately leads to cell death. The membrane-bound temporin1CEa might cause an influx of Oltipraz web extracellular calcium into the intracellular compartment, which led to a rapid increase ofintracellular Ca2+ and ROS concentration 11967625 and a significant transmembrane potential depolarization. The disrupted cell membrane induced by higher concentrations of temporin-1CEa may also permit extracellular peptides to be uptake into cells (as shown by increased intracellular green fluorescence from FITC-labeled temporin-1CEa) to initiate intracellular events and then cause cell death. Given the negative charge of mitochondrial membranes and their structural similarity with bacteria membrane, mitochondria are possibly the preferential intracellular structural target for internalized temporin-1CEa. Previous studies have indicated that AMPs disrupte mitochondrial potential and other mitochondrial functions [16,30,31]. In 15755315 the present study, we hypothesized that the internalized temporin1CEa together with the intracellular calcium overload triggered by endogenous calcium leakage from the intracellular calcium stores (such as TBHQ endoplasmic reticulum) or calcium influxed from extracellular space, cause impairment of mitochondrial structure and function, including an opening of the mitochondrial permeability transition pore (PTP), thus triggered mitochondrial membrane permeabilization and the loss of DwM, and finally activation of cells death [32,33]. However, temporin-1CEa at 20 mM was excluded from cancer cells. Whether the collapse of mitochondrial membrane potential induced by 20 mM temporin1CEa is a result of increased intracellular Ca2+ production orMechanisms of Temporin-1CEa Induced CytotoxicityFigure 8. Disruption of mitochondrial membrane potential in MDA-MB-231 (A) and MCF-7 cells (B) after temporin-1CEa exposure. Mitochondrial membrane potential was measured using the cell-permeable fluorescent cati.E solution (C ). Fluo3-AM green fluorescence was used for evaluation of the cytosolic calcium levels. Each bar represents the mean value from three determinations with the standard deviation (SD). Data (mean 6 SD) with asterisk significantly differ (*p,0.05; **p,0.01) between treatments. doi:10.1371/journal.pone.0060462.gpeptides would induce membrane lipid asymmetry, membrane integrity disruption and enhancement of membrane permeability (as indicated by increased cell surface PS exposure and PI/EthD-1 uptake). Moreover, although temporin-1CEa of 20 mM was excluded from cancer cells, the peptides are still able to trigger intracellular events, including intracellular ROS and calcium ion elevation, transmembrane potential depolarization and loss of mitochondrial membrane potential. The calcium-related mechanisms have been identified to be involved in cell death induced by some certain antimicrobial peptide [29]. In our present study, the increased intracellular calcium concentration induced by 20 mM temporin-1CEa exposure was partlyly mediated by the endogenous calcium released from intracellular stores and have pivotal roles in temporin-1CEa-induced breast cancer cells death, although the detailed intracellular signaling pathway awaits further investigation. When cancer cells were exposed to temporin-1CEa of higher concentrations, temporin-1CEa might induce membrane pore, or directly disrupt cell membranes to lysis. This membrane-disrupting effect resulted in PS exposure, membrane permeablization and even the release of cytoplasmic contents out of the cell, which ultimately leads to cell death. The membrane-bound temporin1CEa might cause an influx of extracellular calcium into the intracellular compartment, which led to a rapid increase ofintracellular Ca2+ and ROS concentration 11967625 and a significant transmembrane potential depolarization. The disrupted cell membrane induced by higher concentrations of temporin-1CEa may also permit extracellular peptides to be uptake into cells (as shown by increased intracellular green fluorescence from FITC-labeled temporin-1CEa) to initiate intracellular events and then cause cell death. Given the negative charge of mitochondrial membranes and their structural similarity with bacteria membrane, mitochondria are possibly the preferential intracellular structural target for internalized temporin-1CEa. Previous studies have indicated that AMPs disrupte mitochondrial potential and other mitochondrial functions [16,30,31]. In 15755315 the present study, we hypothesized that the internalized temporin1CEa together with the intracellular calcium overload triggered by endogenous calcium leakage from the intracellular calcium stores (such as endoplasmic reticulum) or calcium influxed from extracellular space, cause impairment of mitochondrial structure and function, including an opening of the mitochondrial permeability transition pore (PTP), thus triggered mitochondrial membrane permeabilization and the loss of DwM, and finally activation of cells death [32,33]. However, temporin-1CEa at 20 mM was excluded from cancer cells. Whether the collapse of mitochondrial membrane potential induced by 20 mM temporin1CEa is a result of increased intracellular Ca2+ production orMechanisms of Temporin-1CEa Induced CytotoxicityFigure 8. Disruption of mitochondrial membrane potential in MDA-MB-231 (A) and MCF-7 cells (B) after temporin-1CEa exposure. Mitochondrial membrane potential was measured using the cell-permeable fluorescent cati.