Fluorescent indicators for Ca2+based on green fluorescent proteins and calmodulin

Miyawaki, Atsushi; Llopis, Juan; Heim, Roger; McCaffery, J. Michael; Adams, Joseph A.; Ikura, Mitsuhiko; Tsien, Roger Y.

doi:10.1038/42264

Cited by 2,972 publications

(2,360 citation statements)

References 22 publications

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“…The particular disadvantage of chemical Ca 2þ -sensors is the difficulty of controlling cellular localization, for example, the targeting to specific organelles. As an alternative to the chemical sensors, the Tsien lab and others developed genetically encoded Ca 2þ -indicators (GECIs) based on fusions of FPs with calcium responsive elements like calmodulin or troponin [75][76][77][78]. These indicators allow for the dissection of the spatial and temporal control of calcium signaling processes in cells because they are genetically encoded and therefore specifically localized.…”

Section: Localization Of Fluorescent Ca 2þ -Sensors By Chemical Tagsmentioning

confidence: 99%

Chemical tags: Applications in live cell fluorescence imaging

Wombacher

Cornish

2011

Journal of Biophotonics

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Technologies to visualize cellular structures and dynamics enable cell biologists to gain insight into complex biological processes. Currently, fluorescent proteins are used routinely to investigate the behavior of proteins in live cells. Chemical biology techniques for selective labeling of proteins with fluorescent labels have become an attractive alternative to fluorescent protein labeling. In the last ten years the progress in the development of chemical tagging methods have been substantial offering a broad palette of applications for live cell fluorescent microscopy. Several methods for protein labeling have been established, using protein tags, peptide tags and enzyme mediated tagging. This review focuses on the different strategies to achieve the attachment of fluorophores to proteins in live cells and cast light on the advantages and disadvantages of each individual method. Selected experiments in which chemical tags have been successfully applied to live cell imaging will be discussed and evaluated. (© 2011 WILEY‐VCH Verlag GmbH & Co. KGaA, Weinheim)

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Section: Localization Of Fluorescent Ca 2þ -Sensors By Chemical Tagsmentioning

confidence: 99%

Chemical tags: Applications in live cell fluorescence imaging

Wombacher

Cornish

2011

Journal of Biophotonics

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“…Most GECI recognition elements are based on naturally evolved calcium-binding proteins with large Ca 2+ -dependent conformational changes such as calmodulin (CaM) (Miyawaki et al, 1997;Nakai et al, 2001) or troponin-C (TnC) (Heim and Griesbeck, 2004). Wild-type recognition elements have been engineered to improve binding and response properties Garaschuk et al, 2007).…”

Section: Geci Construction Strategiesmentioning

confidence: 99%

“…GECIs can be delivered in a minimally invasive manner to specific cell types or subcellular compartments (Miyawaki et al, 1997). They are compatible with long-term, repeated, in vivo measurements (Hasan et al, 2004).…”

Section: Introductionmentioning

confidence: 99%

Reporting neural activity with genetically encoded calcium indicators

2008

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Genetically encoded calcium indicators (GECIs), based on recombinant fluorescent proteins, have been engineered to observe calcium transients in living cells and organisms. Through observation of calcium, these indicators also report neural activity. We review progress in GECI construction and application, particularly toward in vivo monitoring of sparse action potentials (APs). We summarize the extrinsic and intrinsic factors that influence GECI performance. A simple model of GECI response to AP firing demonstrates the relative significance of these factors. We recommend a standardized protocol for evaluating GECIs in a physiologically relevant context. A potential method of simultaneous optical control and recording of neuronal circuits is presented.

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“…signals are found in the cytosol and different organelles, but these signals are often difficult to measure by conventional fluorescent indicators. The yellow cameleon fluorescent calcium indicators are the most suitable reporters for in vivo detection of calcium because they do not require any cofactors and can be targeted to specific intracellular locations (Miyawaki et al 1997(Miyawaki et al , 1999. Several different variants of yellow cameleons have been constructed but all consist of a tandem fusion of ECFP, a calmodulin domain having four calcium binding sites, a calmodulin binding peptide M13 and EYFP (Miyawaki et al 1997;Varadi and Rutter 2002).…”

Section: Electronic Supplementary Materialsmentioning

confidence: 99%