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. 2015 Oct 22;6(10):e1934. doi: 10.1038/cddis.2015.292

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Copyright © 2015 Macmillan Publishers Limited

Cell Death and Disease is an open-access journal published by Nature Publishing Group. This work is licensed under a Creative Commons Attribution 4.0 International License. The images or other third party material in this article are included in the article's Creative Commons license, unless indicated otherwise in the credit line; if the material is not included under the Creative Commons license, users will need to obtain permission from the license holder to reproduce the material. To view a copy of this license, visit http://creativecommons.org/licenses/by/4.0/

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CM transfer and co-plating experiments to evaluate bystander killing in heterogeneous system. Involvement of sFasL in mediating bystander cytotoxicity. The effector cells (THP-1 MΦ) were treated with 500 nM MMC for 24 h, and then CM was collected after 48 h as described in Materials and Methods. Target HeLa (a) and SiHa (b) cells were incubated with the CM in the presence or absence of MG132 and/or with anti-FasL antibody for 36 h. CM was supplemented with 0.2% FBS to avoid cell death owing to growth factor depletion. Cell survival was further evaluated by MTT assay. Data are mean±S.D., and are representative of three independent experiments performed in triplicates (**P<0.01 when compared with their respective controls). (ci) Apoptotic cell death in target HeLa-EGFP cells in heterogeneous system. Histograms for effector and target cell populations alone or in co-culture are shown by annexin V-PE staining using flow cytometry. 1:Untreated THP-1 MΦ 2: Untreated HeLa-EGFP cells; 3: Untreated effector cells (THP-1 MΦ) were co-plated with target EGFP cells; 4: Effector cells (THP-1 MΦ) were treated with MMC for 24 h, washed with medium and target EGFP cells were co-plated; 5: Untreated effector cells (THP-1 MΦ) were co-plated with target EGFP cells and treated with MG132 for 24 h; 6: Effector cells (THP-1 MΦ) were treated with MMC for 24 h, washed with medium, and target EGFP cells were co-plated and then treated with MG132 for 24 h; 7: Effector cells (THP-1 MΦ) were treated with GW9662 for 2 h followed by addition of MMC for 24 h, and then washed, co-plated with target EGFP cells along with treatment of MG132 and GW9662; 8: Effector cells (THP-1 MΦ) were treated with MMC for 24 h, washed and co-plated with target EGFP cells, and further incubated in the presence of MG132 and anti-TRAIL antibodies; are shown with annexin V-PE positive counts and are indicated as percentages of apoptotic cells; are shown with annexin V-PE positive counts indicated as percentages of apoptotic cells. Upper right quadrant represents proportion of apoptotic bystander target EGFP cells. Effector cells were washed with medium three times before co-plating with the target cells. (cii) The bar graph shows annexin V-PE positive cells in the same experiment. Data are mean±S.D., and are representative of three independent experiments (**P<0.01 when compared with their respective controls). (d) Western blot analysis for PARP cleavage. Target HeLa cells were pretreated with 5 μM MG132 for 2 h. Thereafter, CM collected from MMC-treated effector cells (HeLa and THP-1 MΦ) was added in the presence or absence of MG132 for an additional 24 h. Whole-cell lysates were prepared to perform western blot analysis. The levels of PARP (p116) and its cleaved product (p85) were detected. β-Actin was used as a loading control