V e h ic le M T -II
0
2
4
6
8
*
n = 6 n = 6
Enhanced electrical activity of supraoptic neurones
following systemic melanocortin administration
Luis Paiva, Nancy Sabatier, Gareth Leng, Mike Ludwig.
Centre for Integrative Physiology, University of Edinburgh, Edinburgh, UK.
Introduction
Melanocortins stimulate the central oxytocin systems which regulate social behaviours1. Alterations in central oxytocin has been linked to
neuropsychiatric disorders such as autism and anxiety, and melanocortins have been proposed for therapeutic treatment. Naturally occurring
melanocortins including alpha-melanocyte stimulating hormone (α-MSH) potently stimulate oxytocin release from the dendrites of oxytocin cells, but
inhibit their electrical activity2. α-MSH has a poor penetrance through the blood-brain barrier. Here we investigated whether Melanotan-II (MT-II), a
synthetic melanocortin agonist, affects the electrical activity of supraoptic (SON) oxytocin and vasopressin neurons when given intravenously.
Conclusions
Intravenous (i.v.) administration of MT-II induces neural activation in oxytocin and vasopressin cells of the SON. As oxytocin neurons are electrically
inhibited in response to direct application of melanocortin agonists, the actions of intravenous MT-II are likely to be mediated indirectly.
References
1. Modi et al. 2015. Melanocortin receptor agonists facilitate oxytocin-dependent partner preference formation in the prairie vole.
Neuropsychopharmacology 40: 1856-1865.
2. Sabatier et al. 2003. Alpha-melanocyte-stimulating hormone stimulates oxytocin release from the dendrites of hypothalamic
neurons while inhibiting oxytocin release from their terminals in the neurohypophysis. J Neurosci 23:10351-58.
Femoral
cannulation
MT-II
1mg/kg i.v.
Perfusion
120min 90min Processing for Fos and
oxytocin immunostaining
Adult male SD rat
Pentobarbital anaesthesia
6 rats per group
Methods
Fig. 1. The SON and paraventricular nucleus (PVN) are the main sites of synthesis of oxytocin and
vasopressin in the brain. (A) Coronal section showing immunostaining for Fos (black nuclear) and
oxytocin (brown cytoplasm) in the PVN and SON in a control rat. (B) I.v. injections of MT-II increase
Fos expression in the SON. (D) Fos expression in oxytocin cells of the SON increase following MT-II
administration. (C,E) Fos expression in the SON in vehicle (C) and MT-II (E) treated rats (no oxytocin
staining in these sections). Scale bar = 100µm. Means ± S.E.M.; *P<0.05, Mann-Whitney U test.
MT-II induces Fos expression in the SON
Fig. 2. (A) Typical example of the increase in firing rate in an oxytocin neuron in response to i.v.
administration of MT-II. (B) Mean change in firing rate of 8 oxytocin cells after MT-II i.v. in 30-s bins (±
S.E.M.; *P<0.05, Wilcoxon Signed Rank test).
MT-II enhances electrical activity in
oxytocin neurons when given i.v.
Fig. 3 (A) Typical example of the increase in firing rate in a vasopressin neuron in response to i.v.
administration of MT-II. (B) Mean change in 6 vasopressin cells in response to MT-II i.v. in 10-min bins
(± S.E.M; Wilcoxon Signed Rank test).
A
B
A
B
MT-II also enhances electrical activity
in vasopressin neurons
PVN
SON
D
C
A
25
20
15
10
5
0
Fir
ing
rate
(Sp
ikes/s
)
MT-II
min15 30 45 60 75
5 10 15 20 25 30 min
160
120
80
40
0
Fir
ing
rate
(Sp
ikes/3
0s)
MT-II
0
5
1 0
1 5
2 0
*
n = 6 n = 6
B
0 1 0 2 0 3 0 4 0 5 0
-1
0
1
2
3
4
Mean
ch
an
ge i
n f
irin
g r
ate
(sp
ikes/s
)
Time since MT-II (min)
-5 0 5 1 0-0 .5
0 .0
0 .5
1 .0
1 .5
M T -II
*
Mean
ch
an
ge i
n f
irin
g r
ate
(sp
ikes/s
)
Time since MT-II (min)
E
Femoral
cannulation and
SON exposure
CCK 20 µg/kg i.v.
pharmacological
identification of either
vasopressin and
oxytocin cells
MT-II
1mg/kg i.v.
Adult male SD rat
Urethane anaesthesia
Data analysis
Immunohistochemistry
Electrophysiology
Supported by
Fo
s p
os
itiv
e c
ells
/1
04
µm
2F
os
po
sit
ive
ce
lls
/1
04
µm
2
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