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Mechano-oxidative coupling by mitochondria induces proinflammatory responses in lung venular capillaries
Hideo Ichimura, Kaushik Parthasarathi, Sadiqa Quadri, Andrew C. Issekutz, Jahar Bhattacharya
Hideo Ichimura, Kaushik Parthasarathi, Sadiqa Quadri, Andrew C. Issekutz, Jahar Bhattacharya
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Article Cardiology

Mechano-oxidative coupling by mitochondria induces proinflammatory responses in lung venular capillaries

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Abstract

Elevation of lung capillary pressure causes exocytosis of the leukocyte adhesion receptor P-selectin in endothelial cells (ECs), indicating that lung ECs generate a proinflammatory response to pressure-induced stress. To define underlying mechanisms, we followed the EC signaling sequence leading to P-selectin exocytosis through application of real-time, in situ fluorescence microscopy in lung capillaries. Pressure elevation increased the amplitude of cytosolic Ca2+ oscillations that triggered increases in the amplitude of mitochondrial Ca2+ oscillations and in reactive oxygen species (ROS) production. Responses to blockers of the Ca2+ oscillations and of mitochondrial electron transport indicated that the ROS production was Ca2+ dependent and of mitochondrial origin. A new proinflammatory mechanism was revealed in that pressure-induced exocytosis of P-selectin was inhibited by both antioxidants and mitochondrial inhibitors, indicating that the exocytosis was driven by mitochondrial ROS. In this signaling pathway mitochondria coupled pressure-induced Ca2+ oscillations to the production of ROS that in turn acted as diffusible messengers to activate P-selectin exocytosis. These findings implicate mitochondrial mechanisms in the lung’s proinflammatory response to pressure elevation and identify mitochondrial ROS as critical to P-selectin exocytosis in lung capillary ECs.

Authors

Hideo Ichimura, Kaushik Parthasarathi, Sadiqa Quadri, Andrew C. Issekutz, Jahar Bhattacharya

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Figure 1

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Fluorescence of ECs in situ in a lung venular capillary. (a) Confocal im...
Fluorescence of ECs in situ in a lung venular capillary. (a) Confocal images show a fluorescent EC (arrow). Dotted lines are capillary margins as detected in bright-field images obtained in parallel. Bar = 10 μm. (b) Single EC imaged at high magnification shows mitochondria as fluorescent clumps (arrows). Bar = 2 μm. (c) Effect of saponin (0.01%) treatment. Capillaries were coloaded with dyes and excited alternately at the wavelengths indicated in parentheses under Ca2+-free conditions. Each point is mean ± SE of three determinations. MTG, MitoTracker Green.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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