Mechanisms for PACAP-induced prolactin gene expression in grass carp pituitary cells:
In mammals, pituitary adenylate cyclase-activating polypeptide (PACAP) is a pleiotropic hormone with diverse functions but its role in prolactin (PRL) regulation is highly controversial. To shed light on PRL regulation by PACAP in fish model, grass carp pituitary cells was used as a model to examine the receptor specificity and signal transduction for PACAP modulation of PRL gene expression in the carp pituitary. Using RT-PCR, PACAP-selective PAC-I receptor was detected in carp lactotrophs. In carp pituitary cells, nanomolar doses of PACAP, but not VIP, could elevate PRL secretion and protein production with concurrent rise in PRL mRNA and these stimulatory effects were blocked by PACAP antagonist but not VIP antagonist. PACAP-induced PRL mRNA expression could be mimicked by activating adenylate cyclase (AC), increasing cAMP level by cAMP analog, or increasing intracellular Ca2+ ([Ca2+]i) by Ca2+ ionophore/voltage-sensitive Ca2+ channel (VSCC) activator. PACAP-induced PRL gene expression, however, was attenuated/abolished by suppressing cAMP production, inhibiting PKA activity, blocking [Ca2+]i mobilization and VSCC activation, calmodulin (CaM) antagonism, and inactivation of JNK and CaM Kinase-II (CaMK-II). Similar sensitivity to CaM, JNK and CaMK-II blockade was also noted by substituting cAMP analog for PACAP as the stimulant for PRL mRNA expression. These results, as a whole, provide evidence for the first time that (i) PACAP activation of PAC-I receptor expressed in carp lactotrophs could induce PRL synthesis and secretion, and (ii) PRL production induced by PACAP was mediated by up-regulation of PRL gene expression, presumably via functional coupling of cAMP/PKA-, Ca2+/CaM- and MAPK-dependent cascades.
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