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Spectral imaging of FRET‐based sensors reveals sustained cAMP gradients in three spatial dimensions
Author(s) -
Annamdevula Naga S.,
Sweat Rachel,
Griswold John R.,
Trinh Kenny,
Hoffman Chase,
West Savannah,
Deal Joshua,
Britain Andrea L.,
Jalink Kees,
Rich Thomas C.,
Leavesley Silas J.
Publication year - 2018
Publication title -
cytometry part a
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.316
H-Index - 90
eISSN - 1552-4930
pISSN - 1552-4922
DOI - 10.1002/cyto.a.23572
Subject(s) - förster resonance energy transfer , confocal microscopy , biophysics , confocal , second messenger system , microscopy , fluorescence lifetime imaging microscopy , fluorescence , compartmentalization (fire protection) , intracellular , forskolin , autofluorescence , microbiology and biotechnology , biology , adenylyl cyclase , chemistry , signal transduction , physics , optics , biochemistry , receptor , enzyme
Abstract Cyclic AMP is a ubiquitous second messenger that orchestrates a variety of cellular functions over different timescales. The mechanisms underlying specificity within this signaling pathway are still not well understood. Several lines of evidence suggest the existence of spatial cAMP gradients within cells, and that compartmentalization underlies specificity within the cAMP signaling pathway. However, to date, no studies have visualized cAMP gradients in three spatial dimensions (3D: x , y , z ).This is in part due to the limitations of FRET‐based cAMP sensors, specifically the low signal‐to‐noise ratio intrinsic to all intracellular FRET probes. Here, we overcome this limitation, at least in part, by implementing spectral imaging approaches to estimate FRET efficiency when multiple fluorescent labels are used and when signals are measured from weakly expressed fluorescent proteins in the presence of background autofluorescence and stray light. Analysis of spectral image stacks in two spatial dimensions (2D) from single confocal slices indicates little or no cAMP gradients formed within pulmonary microvascular endothelial cells (PMVECs) under baseline conditions or following 10 min treatment with the adenylyl cyclase activator forskolin. However, analysis of spectral image stacks in 3D demonstrates marked cAMP gradients from the apical to basolateral face of PMVECs. Results demonstrate that spectral imaging approaches can be used to assess cAMP gradients—and in general gradients in fluorescence and FRET—within intact cells. Results also demonstrate that 2D imaging studies of localized fluorescence signals and, in particular, cAMP signals, whether using epifluorescence or confocal microscopy, may lead to erroneous conclusions about the existence and/or magnitude of gradients in either FRET or the underlying cAMP signals. Thus, with the exception of cellular structures that can be considered in one spatial dimension, such as neuronal processes, 3D measurements are required to assess mechanisms underlying compartmentalization and specificity within intracellular signaling pathways.