Fig. 1.
Fig. 1. As2O3or IFN-α + As2O3 induced apoptosis in HTLV-1 infected cell lines. / (A) FACS, (B) DAPI staining, or (C) ΔΨm collapse analyses of HTLV-1–infected cells after various treatments. (A) MT-2 cells were treated with buffer control, IFN-α, As2O3, or IFN-α + As2O3 for 60 hours. Cells were then harvested and washed in PBS without Ca++/Mg2+. They were stained using the Vybrant Apoptosis kit. Annexin V conjugated to fluorescein allowed the identification of apoptotic cells, whereas PI allowed the identification of dead cells. Apoptotic cells were annexin V+ and PI−. (B) DAPI staining of MT-2 cells after the same treatments. Magnification × 40. (C) ΔΨm Collapse was measured with the Apoalert Mitochondrial Membrane Sensor kit. Results are representative of at least 2 experiments performed with different HTLV-1–transformed cells.

As2O3or IFN-α + As2O3 induced apoptosis in HTLV-1 infected cell lines.

(A) FACS, (B) DAPI staining, or (C) ΔΨm collapse analyses of HTLV-1–infected cells after various treatments. (A) MT-2 cells were treated with buffer control, IFN-α, As2O3, or IFN-α + As2O3 for 60 hours. Cells were then harvested and washed in PBS without Ca++/Mg2+. They were stained using the Vybrant Apoptosis kit. Annexin V conjugated to fluorescein allowed the identification of apoptotic cells, whereas PI allowed the identification of dead cells. Apoptotic cells were annexin V+ and PI. (B) DAPI staining of MT-2 cells after the same treatments. Magnification × 40. (C) ΔΨm Collapse was measured with the Apoalert Mitochondrial Membrane Sensor kit. Results are representative of at least 2 experiments performed with different HTLV-1–transformed cells.

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