Fluorescence microscopy studies with a fluorescent glibenclamide derivative, a high-affinity blocker of pancreatic β-cell ATP-sensitive K + currents

Abstract

Hypoglycemic sulfonylureas (e.g. tolbutamide, glibenclamide) exert their stimulatory effects on pancreatic β-cells by closure of ATP-sensitive K + (K ATP) channels. Pancreatic K ATP channels are composed of two subunits, a pore-forming inwardly rectifying K + channel (Kir6.2) subunit and a regulatory subunit (the sulfonylurea receptor of subtype 1 (SUR1)) in a (SUR1/Kir6.2) 4 stoichiometry. The aim of the present study was to characterize the interaction of green-fluorescent 3-[3-(4,4 difluoro-5,7-dimethyl-4-bora-3 a,4 a-diaza- S-indacen-3-yl)propanamido] glibenclamide (Bodipy-glibenclamide) with pancreatic β-cell K ATP channels using patch-clamp and fluorescence microscopy techniques. Bodipy-glibenclamide inhibited K ATP currents from the clonal insulinoma cell line RINm5F half-maximally at a concentration of 0.6 nM. Using laser-scanning confocal microscopy Bodipy-glibenclamide was shown to induce a diffuse fluorescence across the RINm5F cell, but only about 17% of total Bodipy-glibenclamide-induced fluorescence intensity in RINm5F cells was due to specific binding to SUR1. Using fluorescence correlation spectroscopy, it could be demonstrated that the fluorescence label contributes to the protein binding and, therefore, possibly also to the non-specific binding of Bodipy-glibenclamide observed in RINm5F cells. Specific binding of Bodipy-glibenclamide to SUR1 in RINm5F cells might be localized to different intracellular structures (nuclear envelope, endoplasmic reticulum, Golgi compartment, insulin secretory granules) as well as to the plasma membrane. In conclusion, Bodipy-glibenclamide is a high-affinity blocker of pancreatic β-cell K ATP currents and can be used for visualizing SUR1 in intact pancreatic β-cells, although non-specific binding must be taken into account in confocal microscopy experiments on intact β-cells.