Altering integrin engagement regulates membrane localization of Kir2.1 channels.
How ion channels localize and distribute on the cell membrane remains incompletely understood. We show that interventions that vary cell adhesion proteins and cell size also affect the membrane current density of inward-rectifier K+ channels (Kir2.1; encoded by KCNJ2) and profoundly alter the action potential shape of excitable cells. By using micropatterning to manipulate the localization and size of focal adhesions (FAs) in single HEK293 cells engineered to stably express Kir2.1 channels or in neonatal rat cardiomyocytes, we establish a robust linear correlation between FA coverage and the amplitude of Kir2.1 current at both the local and whole-cell levels. Confocal microscopy showed that Kir2.1 channels accumulate in membrane proximal to FAs. Selective pharmacological inhibition of key mediators of protein trafficking and the spatially dependent alterations in the dynamics of Kir2.1 fluorescent recovery after photobleaching revealed that the Kir2.1 channels are transported to the cell membrane uniformly, but are preferentially internalized by endocytosis at sites that are distal from FAs. Based on these results, we propose adhesion-regulated membrane localization of ion channels as a fundamental mechanism of controlling cellular electrophysiology via mechanochemical signals, independent of the direct ion channel mechanogating.
Duke Scholars
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Related Subject Headings
- Rats, Sprague-Dawley
- Rats
- Potassium Channels, Inwardly Rectifying
- Membrane Potentials
- Ion Channel Gating
- Integrins
- Humans
- HEK293 Cells
- Female
- Endocytosis
Citation
Published In
DOI
EISSN
ISSN
Publication Date
Volume
Issue
Start / End Page
Related Subject Headings
- Rats, Sprague-Dawley
- Rats
- Potassium Channels, Inwardly Rectifying
- Membrane Potentials
- Ion Channel Gating
- Integrins
- Humans
- HEK293 Cells
- Female
- Endocytosis