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Br J Pharmacol. 2011 Aug;163(8):1605-25. doi: 10.1111/j.1476-5381.2010.00988.x.

Imaging calcium signals in vivo: a powerful tool in physiology and pharmacology.

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1
Section on Cell Biology and Signal Transduction, Laboratory of Cellular and Molecular Neurophysiology, National Institute of Child Health and Human Development/NIH, 49 Convent Drive, Bethesda, MD 20892-4480, USA. james@helix.nih.gov

Abstract

The design and engineering of organic fluorescent Ca(2+) indicators approximately 30 years ago opened the door for imaging cellular Ca(2+) signals with a high degree of temporal and spatial resolution. Over this time, Ca(2+) imaging has revolutionized our approaches for tissue-level spatiotemporal analysis of functional organization and has matured into a powerful tool for in situ imaging of cellular activity in the living animal. In vivo Ca(2+) imaging with temporal resolution at the millisecond range and spatial resolution at micrometer range has been achieved through novel designs of Ca(2+) sensors, development of modern microscopes and powerful imaging techniques such as two-photon microscopy. Imaging Ca(2+) signals in ensembles of cells within tissue in 3D allows for analysis of integrated cellular function, which, in the case of the brain, enables recording activity patterns in local circuits. The recent development of miniaturized compact, fibre-optic-based, mechanically flexible microendoscopes capable of two-photon microscopy opens the door for imaging activity in awake, behaving animals. This development is poised to open a new chapter in physiological experiments and for pharmacological approaches in the development of novel therapies.

PMID:
20718728
PMCID:
PMC3166690
DOI:
10.1111/j.1476-5381.2010.00988.x
[Indexed for MEDLINE]
Free PMC Article
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