Characterization of Membrane‐Associated Peptidase Activities Expressed by Endothelial Cells of the Ovine Median Eminence

The capillary endothelial cells of the median eminence represent a potential site for the degradation/modification of both circulating and hypothalamic peptides passing through the hypophysial portal system toward the pituitary. This study examines endothelial cell peptidase expression in vitro by monitoring the metabolism of gonadotropin‐releasing hormone (GnRH) by cultured endothelial cells from sheep median eminence. Cleavage of GnRH by median eminence endothelial cell membranes generated GnRH 1–5 as the primary stable product, which was then degraded to GnRH 1–3 and free amino acids. Degradation of GnRH was completely inhibited by TPCK, ZnCI 2 and N‐ethylmaleimide, and partially inhibited by EDTA and by a specific inhibitor of the metalloendopeptidase EC 3.4.24.15, CFP‐AAY‐pAB. Interestingly, an increase in GnRH 1–9 production was seen with the latter inhibitors, suggesting a two‐step mechanism of GnRH degradation involving a primary cleavage at the Pro 9 ‐Gly 10 ‐NH 2 bond, inhibitable by TPCK, ZnCI 2 , and NEM, followed by cleavage by EC 3.4.24.15 to generate GnRH 1–5 . Phosphoramidon and angiotensin converting enzyme inhibitors (as well as other non‐specific inhibitors) were without effect, indicating that endopeptidase EC 3.4.24.11 and angiotensin converting enzyme are not involved. Neither bovine aortic endothelial cell nor AtT‐20 cell membranes exhibited this pattern of peptidase activity. Degradation of GnRH by intact median eminence endothelial cells in culture was also observed, suggesting an extracellular orientation for these enzymes; the potential role of such peptidases in the fine regulation of both pituitary function and local blood flow is currently under investigation.