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Original Studies |
Maternal Health Research Centre (E.-C.C., J.T.F., R.S.), Endocrine Unit, John Hunter Hospital, Newcastle, N.S.W. 2310, Australia; and Department of Neurobiology (X.N.), Second Military Medical University, Shanghai 200433, P.R. China
Address all correspondence and requests for reprints to: Prof. Roger Smith, Maternal Health Research Centre, Endocrine Unit, Locked Bag 1, Hunter Regional Mail Centre, Newcastle, N.S.W. 2310, Australia. E-mail: mdrsm{at}mail.newcastle.edu.au
Nitric oxide (NO) plays an important role in many cell-cell signaling
systems, but its mechanism of action is variable. We have previously
reported that NO reduces secretion of the peptide hormone, CRH, from
cultured placental cells and the perfused placenta. Because placental
CRH production seems linked to human parturition, we wished to explore
the mechanism of action of NO in this setting in more detail. We report
here that in the placenta, NO specifically inhibited CRH exocytosis,
not synthesis, and that endogenous NO affects this process.
Cytotrophoblasts were prepared from term human placentas and cultured
as monolayers. CRH immunoreactivity in the cell supernatants and cell
extracts were measured by RIA. CRH messenger RNA was determined by
Northern blot analysis. Sodium nitroprusside (SNP; 1100 µmol/L) and
S-nitroso-N-acetyl-penicillamine (SNAP; 1100
µmol/L), NO donors, significantly reduced basal CRH concentration in
the media, while increasing the concentration of CRH in the cells
(P < 0.01), suggesting that exocytosis of CRH was
inhibited. These effects could be attenuated by the NO scavenger
hemoglobin (20 µg/mL). KCl (45 mmol/L), which causes exocytosis by
depolarizing the cell membrane, increased CRH release by 2- to 3-fold,
and this was inhibited by SNP. Basal release of CRH was augmented by
the NO synthase competitive inhibitor
N
-L-arginine methyl ester (1 mmol/L;
P < 0.01) and the guanylate cyclase inhibitor,
LY83583 (1 µmol/L; P < 0.01). The inhibitory
effect of SNP was also blocked by LY83583. CRH messenger RNA content
did not change when the placental cells were incubated with SNP,
N
-L-arginine methyl ester, and LY83583 for 6
and 24 h, and this was consistent with studies showing that total
CRH immunoreactivity (cells plus media) did not change in the presence
of SNP. These studies indicate that exogenous NO inhibits CRH
exocytosis, rather than biosynthesis, by human trophoblasts and that
endogenous NO has tonic inhibitory effects on CRH release by these
cells. The inhibitory effect of NO on basal and stimulated CRH release
by placental trophoblasts seems to be a guanylate cyclase-mediated
inhibition of exocytosis.
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