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Secure an arteriolar endothelial tube harvested from a mouse brain in a chamber with a continuous buffer flow.
Place the chamber in a recording setup.
Introduce a calcium-sensitive fluorescent dye. Incubate to allow cellular uptake of the dye.
Wash to remove any non-internalized dye.
Insert an electrode into an endothelial cell and record the resting membrane potential.
Raise the bath temperature to a physiological temperature to facilitate intracellular calcium binding to the dye.
Excite the dye and measure fluorescence to quantify baseline cellular calcium levels.
Introduce a drug that binds to specific G-protein-coupled receptors on the endothelial cells, initiating a signaling cascade.
This cascade releases calcium ions from the endoplasmic reticulum into the cytoplasm, enhancing calcium-dye binding and fluorescence.
Elevated cytoplasmic calcium levels also activate potassium channels, facilitating potassium ion efflux and decreasing membrane potential.
Record the data.
Increased fluorescence and decreased membrane potential indicate a functional endothelial tube.
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