Itive, Q4 quadrant), and cells with interrupted membrane integrity (FITC-annexin V positive and PI positive, Q2 quadrant). The FACS analysis LY2409021 cost indicated that while the viable cells captured in Q3 quadrant was reduced, the cells captured in Q2 or Q4 quadrant was increased (Fig. 3A for MDA-MB-231 and Fig.3B for MCF-7 cells, respectively). These results indicated that temporin-1CEa could affect cancer cells viability by disrupting their membrane integrity (as shown by the cell surface PS exposure) and increasing membrane permeability (as indicated by uptake of PI into cells). In addition, the cells sorting data also suggested two cancer cell lines exerted different response manners to temporin1CEa exposure. Consistent with the in vitro cytotoxicity assay, MCF-7 cells were more susceptible than MDA-MB-231 cells as indicated by the lower levels of viable cells in Q3 quadrant. Moreover, the temporin-1CEa-treated MCF-7 cells seemed to be more permeable for PI as indicated by higher Q2 values (Fig. 3B), while MDA-MB-231 cells preferred to be affected on the cell surface as indicated by higher Q4 value (Fig. 3A).Temporin-1CEa Induces Enhancement of Membrane PermeabilityTo confirm the membrane permeablizing effect of temporin1CEa on MDA-MB-231 and MCF-7 cells, calcein AM and ethidium homodimer (EthD-1) were used. Live cells have intracellular esterases that convert nonfluorescent, cell-permeable calcein AM to the intensely fluorescent green calcein, which is retained within the live cells with intact membrane. EthD-1 is excluded by the intact plasma membrane of live cells. However, in membrane-disrupted or dead cells with enhanced membrane-permeability, EthD-1 enters into intracellular space of cells and produces bright-red SPDP Crosslinker web fluorescence when bound to nucleic acids. Therefore, an increased fluorescence intensity of EthD-1 or a decreased fluorescence intensity of calcein means enhanced membrane permeability and interrupted membrane integrity. As shown in Fig. 4, after one-hour exposure of temporin-1CEa, the fluorescence intensity of calcein was reduced (Fig. 4A-B); meanwhile, the fluorescence intensity of EthD-1 was increased in cells (Fig. 4C-D). These results suggested that temporin-1CEa disrupted the cell membranes of MDA-MB-231 and MCF-7 cells leading to an increase in membrane permeability. Moreover, in the absence or presence of temporin-1CEa, the MDA-MB-231 cells showed a lower permeability for the membrane-permeable calcein AM than MCF-7 cells, as indicated 15755315 by the lower level of intracellular calcein fluorescence intensity.Temporin-1CEa Induces Morphological ChangesMorphological examination via scanning electron microscopy (Fig. 2A) or transmission electron microscopy (Fig. 2B) revealed that one hour incubation of various concentrations of temporin1CEa induced dramatic morphological changes in both MDAMB-231 and MCF-7 breast cancer cells. While untreated control cells showed an intact membrane and smooth surface, the temporin-1CEa-treated cancer cells membrane were shriveled, invaginated and disrupted, which may in turn resulted in irreversible cytolysis and finally death of the target cells.Temporin-1CEa Induces Cell Surface Exposure of Phosphatidylserine and Disruption of Plasma Membrane Integrity in MDA-MB-231 CellsPhosphatidylserine (PS) exposure on the surface of cells has been considered a characteristic feature of membrane disruption or cell death [19]. When the plasma membrane loses its integrity, PS originally exist in the inner leaf.Itive, Q4 quadrant), and cells with interrupted membrane integrity (FITC-annexin V positive and PI positive, Q2 quadrant). The FACS analysis indicated that while the viable cells captured in Q3 quadrant was reduced, the cells captured in Q2 or Q4 quadrant was increased (Fig. 3A for MDA-MB-231 and Fig.3B for MCF-7 cells, respectively). These results indicated that temporin-1CEa could affect cancer cells viability by disrupting their membrane integrity (as shown by the cell surface PS exposure) and increasing membrane permeability (as indicated by uptake of PI into cells). In addition, the cells sorting data also suggested two cancer cell lines exerted different response manners to temporin1CEa exposure. Consistent with the in vitro cytotoxicity assay, MCF-7 cells were more susceptible than MDA-MB-231 cells as indicated by the lower levels of viable cells in Q3 quadrant. Moreover, the temporin-1CEa-treated MCF-7 cells seemed to be more permeable for PI as indicated by higher Q2 values (Fig. 3B), while MDA-MB-231 cells preferred to be affected on the cell surface as indicated by higher Q4 value (Fig. 3A).Temporin-1CEa Induces Enhancement of Membrane PermeabilityTo confirm the membrane permeablizing effect of temporin1CEa on MDA-MB-231 and MCF-7 cells, calcein AM and ethidium homodimer (EthD-1) were used. Live cells have intracellular esterases that convert nonfluorescent, cell-permeable calcein AM to the intensely fluorescent green calcein, which is retained within the live cells with intact membrane. EthD-1 is excluded by the intact plasma membrane of live cells. However, in membrane-disrupted or dead cells with enhanced membrane-permeability, EthD-1 enters into intracellular space of cells and produces bright-red fluorescence when bound to nucleic acids. Therefore, an increased fluorescence intensity of EthD-1 or a decreased fluorescence intensity of calcein means enhanced membrane permeability and interrupted membrane integrity. As shown in Fig. 4, after one-hour exposure of temporin-1CEa, the fluorescence intensity of calcein was reduced (Fig. 4A-B); meanwhile, the fluorescence intensity of EthD-1 was increased in cells (Fig. 4C-D). These results suggested that temporin-1CEa disrupted the cell membranes of MDA-MB-231 and MCF-7 cells leading to an increase in membrane permeability. Moreover, in the absence or presence of temporin-1CEa, the MDA-MB-231 cells showed a lower permeability for the membrane-permeable calcein AM than MCF-7 cells, as indicated 15755315 by the lower level of intracellular calcein fluorescence intensity.Temporin-1CEa Induces Morphological ChangesMorphological examination via scanning electron microscopy (Fig. 2A) or transmission electron microscopy (Fig. 2B) revealed that one hour incubation of various concentrations of temporin1CEa induced dramatic morphological changes in both MDAMB-231 and MCF-7 breast cancer cells. While untreated control cells showed an intact membrane and smooth surface, the temporin-1CEa-treated cancer cells membrane were shriveled, invaginated and disrupted, which may in turn resulted in irreversible cytolysis and finally death of the target cells.Temporin-1CEa Induces Cell Surface Exposure of Phosphatidylserine and Disruption of Plasma Membrane Integrity in MDA-MB-231 CellsPhosphatidylserine (PS) exposure on the surface of cells has been considered a characteristic feature of membrane disruption or cell death [19]. When the plasma membrane loses its integrity, PS originally exist in the inner leaf.
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