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J Appl Physiol 102: 1255-1264, 2007. First published November 9, 2006; doi:10.1152/japplphysiol.00786.2006 Free Article
8750-7587/07 $8.00
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INVITED REVIEW

HIGHLIGHTED TOPIC
Physiological Imaging of the Lung

Real-time lung microscopy

Wolfgang M. Kuebler,1 Kaushik Parthasarathi,2 Jens Lindert,2 and Jahar Bhattacharya2,3

1Lung and Circulatory Research Laboratory, Institute of Physiology, Charité-Universitätsmedizin, Berlin, Germany; and 2Lung Biology Laboratory, Department of Physiology and Cellular Biophysics, and 3Department of Medicine, College of Physicians and Surgeons, Columbia University, and St. Luke's-Roosevelt Hospital Center, New York, New York

Although proinflammatory cell signaling in the alveolo-capillary region predisposes to acute lung injury, key cell-signaling mechanisms remain inadequately understood. Alveolo-capillary inflammation is likely to involve coordinated signaling among cells of different phenotypes. For example, migration of inflammatory cells into the alveolus might entail coordinated signaling between adjoining alveolar epithelial and microvascular endothelial cells. The popular cultured cell experimental strategy fails to replicate this multicellular environment. Cultured lung cells, both alveolar and endothelial, undergo phenotypic transformations; hence they might inadequately reflect innate responses of native cells. Consequently, new approaches are required for the investigation of cell signaling in the native setting. Here we summarize new developments in classical intravital microscopy and discuss real-time fluorescence imaging as a novel technique for studying second-messenger mechanisms in the alveolo-capillary region.

calcium ion; mitochondria; mitochondrial calcium ion; reactive oxygen species; nitric oxide; P-selectin; surfactant



Address for reprint requests and other correspondence: J. Bhattacharya, St. Luke's-Roosevelt Hospital Center, AJA 509, 1000 10thAve., New York, New York 10019 (e-mail: jb39{at}columbia.edu)




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