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Volume 17, Number 2,
Issue of January 15, 1997
pp. 563-575
Copyright ©1997 Society for Neuroscience
Cellular Localization of the Prohormone Convertases in the
Hypothalamic Paraventricular and Supraoptic Nuclei: Selective
Regulation of PC1 in Corticotrophin-Releasing Hormone Parvocellular
Neurons Mediated by Glucocorticoids
Received May 29, 1996; revised Oct. 7, 1996; accepted Oct. 24, 1996.
Weijia Dong,
Bertolt Seidel,
Mieczyslaw Marcinkiewicz,
Michel Chrétien,
Nabil G. Seidah, and
Robert Day
J. A. DeSève Laboratory of Biochemical Neuroendocrinology,
Clinical Research Institute of Montréal, Montréal,
Québec, Canada H2W 1R7
The prohormone convertases (PCs) are processing enzymes that
activate proproteins via cleavage at specific single or pairs of basic
residues. The hypothalamic paraventricular nucleus (PVN) and supraoptic
nucleus (SON) are primary sites of biosynthesis of several
neuroendocrine hormone precursors, including provasopressin (pro-AVP),
pro-oxytocin (pro-OT), and procorticotrophin-releasing hormone
(pro-CRH), which require post-translational processing to yield active
products. Using in situ hybridization, we observed PC1
and PC5 mRNAs in PVN and SON magnocellular neurons, while PC2 mRNA was
observed in both magnocellular and parvocellular PVN neurons as well as
magnocellular SON neurons. Similar to furin, PC7 mRNA was expressed
throughout the PVN and SON, whereas PACE4 mRNA levels were
undetectable. Both immunohistochemical and Western blot studies were
performed to demonstrate the presence of PC proteins and forms in the
PVN and SON. Using double-labeling in situ
hybridization, we examined the cellular colocalization of each PC mRNA
with pro-AVP, pro-OT, and pro-CRH mRNAs in PVN and SON. PC1 mRNA was
colocalized with both AVP and OT mRNA in PVN and SON magnocellular
neurons. All AVP, OT, and CRH neurons expressed PC2. In contrast, PC5
mRNA was colocalized only with OT mRNA. We examined the effects of
adrenalectomy (ADX) on PVN PC mRNA levels. PC1 mRNA levels were
increased selectively within CRH/AVP parvocellular neurons but were
unchanged in PVN magnocellular AVP or OT neurons. These results
established the anatomical organization of each convertase and
proneuropeptide substrates in the PVN and SON and suggested potential
roles for each enzyme under resting and stimulated conditions.
Key words:
in situ hybridization;
processing;
neuropeptides;
hypothalamic-pituitary-adrenal axis;
proprotein
convertases;
immunohistochemistry
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