Optical estimation of absolute membrane potential using fluorescence lifetime imaging

Author:

Lazzari-Dean Julia R1ORCID,Gest Anneliese MM1,Miller Evan W123ORCID

Affiliation:

1. Department of Chemistry, University of California, Berkeley, Berkeley, United States

2. Department of Molecular & Cell Biology, University of California, Berkeley, Berkeley, United States

3. Helen Wills Neuroscience Institute, University of California, Berkeley, Berkeley, United States

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.

Funder

National Science Foundation

National Institutes of Health

Alfred P. Sloan Foundation

March of Dimes Foundation

Publisher

eLife Sciences Publications, Ltd

Subject

General Immunology and Microbiology,General Biochemistry, Genetics and Molecular Biology,General Medicine,General Neuroscience

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