Hypertension, Vol 9, 295-303, Copyright © 1987 by American Heart Association
A Luckhoff, R Busse, I Winter and E Bassenge
Cultured bovine endothelial cells were grown on microcarrier beads. Columns
(0.2 ml) packed with microcarriers were perfused with oxygenated (20% O2)
Tyrode's solution containing indomethacin (10 microM), and the effluent was
passed through precontracted, endothelium- denuded detector arteries. When
the endothelial cells were stimulated with bradykinin (3-100 nM), adenosine
5'-triphosphate (0.3-30 microM), or calcium ionophore A23187 (10-300 nM),
they released dose-dependently a nonprostanoid compound that dilated the
detector vessel. The factor, probably identical to the endothelium-derived
relaxing factor of native endothelium, evoked dilations of the same
magnitude in different types of detector vessels (rabbit thoracic aorta,
rabbit femoral artery, canine coronary artery). However, this relaxant
factor was significantly more effective in arteries precontracted by
norepinephrine or serotonin than in arteries precontracted by potassium
depolarization. Thus, its dilator action resembles that of the
nitrovasodilators. The factor is labile, with an apparent half-life in the
range of 20 to 30 seconds. Its dilator potency was inhibited by
dithiothreitol (0.2 mM), metyrapone (0.2 mM), nordihydroguaiaretic acid (20
microM), and hemoglobin (1 microM), all of which apparently inactivated the
factor. Synthesis or release (or both) of the relaxant factor was abolished
by methylene blue (1 microM). High PO2 levels (greater than 400 mm Hg) in
the perfusate markedly reduced the release of the relaxant factor from the
cultured cells. This study demonstrates that a vascular relaxant factor is
released from endothelial cells in monoculture by adenosine
5'-triphosphate, bradykinin, and A23187 and establishes such a culture as a
useful tool for analyzing the mechanisms of endothelium-dependent
vasomotion.
ARTICLES
Characterization of vascular relaxant factor released from cultured endothelial cells
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