Literature DB >> 31545164

Optical estimation of absolute membrane potential using fluorescence lifetime imaging.

Julia R Lazzari-Dean1, Anneliese Mm Gest1, Evan W Miller1,2,3.   

Abstract

All cells maintain ionic gradients across their plasma membranes, producing transmembrane potentials (Vmem). Mounting evidence suggests a relationship between resting Vmem and the physiology of non-excitable cells with implications in diverse areas, including cancer, cellular differentiation, and body patterning. A lack of non-invasive methods to record absolute Vmem limits our understanding of this fundamental signal. To address this need, we developed a fluorescence lifetime-based approach (VF-FLIM) to visualize and optically quantify Vmem with single-cell resolution in mammalian cell culture. Using VF-FLIM, we report Vmem distributions over thousands of cells, a 100-fold improvement relative to electrophysiological approaches. In human carcinoma cells, we visualize the voltage response to growth factor stimulation, stably recording a 10-15 mV hyperpolarization over minutes. Using pharmacological inhibitors, we identify the source of the hyperpolarization as the Ca2+-activated K+ channel KCa3.1. The ability to optically quantify absolute Vmem with cellular resolution will allow a re-examination of its signaling roles.
© 2019, Lazzari-Dean et al.

Entities:  

Keywords:  biochemistry; cellular physiology; chemical biology; fluorescent indicators; human; membrane potential; physics of living systems

Mesh:

Year:  2019        PMID: 31545164      PMCID: PMC6814365          DOI: 10.7554/eLife.44522

Source DB:  PubMed          Journal:  Elife        ISSN: 2050-084X            Impact factor:   8.140


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