Live cell imaging using confocal microscopy induces intracellular calcium transients and cell death

被引:84
作者
Knight, MM [1 ]
Roberts, SR [1 ]
Lee, DA [1 ]
Bader, DL [1 ]
机构
[1] Univ London Queen Mary Coll, Interdisciplinary Res Ctr, Biomed Mat & Med Engn Div, Dept Engn, London E1 4NS, England
来源
AMERICAN JOURNAL OF PHYSIOLOGY-CELL PHYSIOLOGY | 2003年 / 284卷 / 04期
关键词
photoactivation; free radicals; reactive oxygen species; oxygen; chondrocyte;
D O I
10.1152/ajpcell.00276.2002
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Isolated chondrocytes stained with fluo 4-AM and visualized using standard confocal microscopy techniques exhibited Ca2+ transients and oscillations. Decreasing the power of the laser light decreased the percentage of cells exhibiting these Ca2+ signals. Treatment with the antioxidant ascorbate reduced the Ca2+ response, suggesting that it was mediated by light-induced release of reactive oxygen species (ROS). Cell viability 24 h after the 1-h confocal imaging period was similar to90% for cells that were neither fluorescently stained nor subjected to laser excitation. By contrast, fluorescently stained cells imaged for 1 h exhibited greatly reduced viability. Treatment with ascorbate reduced the level of cell death, suggesting that the effect was mediated by release of exogenous ROS associated with the interaction of light and the fluorochrome. Ca2+ oscillations were not always associated with cell death, suggesting that separate light-sensitive pathways mediate the two processes. Light-activated Ca2+ signaling may trigger alterations in numerous cell processes and thereby represent an important and hitherto overlooked artifact in fluorescent microscopy of viable cells.
引用
收藏
页码:C1083 / C1089
页数:7
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