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1 Department of Internal Medicine,
Endothelin (ET), a
vasoconstrictive peptide, is known to have a variety of biological
actions. Although ET is released by vascular endothelial cells, other
cell populations also have been reported to synthesize and release ET.
In this study, we examined whether ET is synthesized by intestinal
epithelial cells and whether it affects induction of epithelial cell
proliferation by interleukin-2 (IL-2). Subconfluent monolayers of
intestinal epithelial cells (IEC-6 and IEC-18) were maintained in
serum-free medium before addition of rat IL-2. Both IEC-6 and IEC-18
cells released ET-1 into the medium under unstimulated conditions, as
determined by a sandwich ELISA. IL-2 significantly enhanced ET-1
release in a time-dependent manner. ET-3 was not detectable in the
culture media of either cell line. Expression of ET-1 and ET-3 mRNA in epithelial cells was assessed by competitive PCR. Both cell lines were
shown to express ET-1 mRNA, but no ET-3 mRNA was detected. IL-2
treatment enhanced ET-1 mRNA expression by both IEC-6 and IEC-18 cells.
Both cell lines also expressed mRNA for
ETA and ETB receptor subtypes. When cell
proliferation was assessed, exogenous ET-1 induced a slight
proliferative response in both types of cells that was consistent and
significant at low ET-1 concentrations; cell growth was inhibited at a
higher concentration (10
7
M). IL-2 produced a significant proliferative response in both cell
lines. However, the addition of ET-1
(10
7 M) to culture media
attenuated the IL-2-induced increase in cell proliferation.
ETA-receptor antagonists
significantly enhanced cellular proliferation, suggesting involvement
of the ETA receptor in modulation
of IL-2-induced intestinal epithelial cell growth.
ETA receptor; mRNA expression
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