Characterization and imaging of A6 epithelial cell clones expressing fluorescently labeled ENaC subunits

Author:

Blazer-Yost Bonnie L.1,Butterworth Michael2,Hartman Amy D.1,Parker Gretchen E.1,Faletti Carla J.1,Els Willem J.2,Rhodes Simon J.1

Affiliation:

1. Department of Biology, Indiana University-Purdue University Indianapolis, Indianapolis, Indiana 46202; and

2. Department of Anatomy and Cell Biology, University of Cape Town Medical School, Cape Town, South Africa

Abstract

A6 model renal epithelial cells were stably transfected with enhanced green fluorescent protein (EGFP)-tagged α- or β-subunits of the epithelial Na+channel (ENaC). Transfected RNA and proteins were both expressed in low abundance, similar to the endogenous levels of ENaC in native cells. In living cells, laser scanning confocal microscopy revealed a predominately subapical distribution of EGFP-labeled subunits, suggesting a readily accessible pool of subunits available to participate in Na+ transport. The basal level of Na+ transport in the clonal lines was enhanced two- to fourfold relative to the parent line. Natriferic responses to insulin or aldosterone were similar in magnitude to the parent line, while forskolin-stimulated Na+ transport was 64% greater than control in both the α- and β-transfected lines. In response to forskolin, EGFP-labeled channel subunits traffic to the apical membrane. These data suggest that channel regulators, not the channel per se, form the rate-limiting step in response to insulin or aldosterone stimulation, while the number of channel subunits is important for basal as well as cAMP-stimulated Na+transport.

Publisher

American Physiological Society

Subject

Cell Biology,Physiology

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