Vol. 275, Issue 4, R1003-R1012, October 1998
Acidic fibroblast growth factor activates adrenomedullary
secretion and sympathetic outflow in rats
Itsuro
Matsumoto1,
Akira
Niijima2,
Yutaka
Oomura3,
Kazuo
Sasaki4,
Katsuhiko
Tsuchiya5, and
Tadaomi
Aikawa1
1 Department of Physiology,
Nagasaki University School of Medicine and
5 Department of Environmental
Physiology, Institute of Tropical Medicine, Nagasaki University,
Nagasaki 852; 2 Department of
Physiology, Niigata University School of Medicine, Niigata 951;
3 Institute of Bio-Active Science,
Nippon Zoki Pharmaceutical Company, Yashiro, Hyogo 673-14; and
4 Division of Bio-Information
Engineering, Faculty of Engineering, Toyama University, Toyama 930, Japan
 |
ABSTRACT |
Effects of
exogenous acidic fibroblast growth factor (aFGF), which is increased in
the brain by food intake, on the plasma levels of catecholamines and on
sympathetic efferent outflow were examined in anesthetized rats. A
guide cannula was inserted into the cerebral third ventricle, and a
vascular indwelling catheter was inserted into the right atrium from
the jugular vein. Plasma epinephrine (Epi) and norepinephrine
(NE) increased markedly in a dose-dependent manner for up
to 120 min after intracerebroventricular or intravenous
administration of aFGF (6-667 fmol/rat). Concomitant increases
occurred in the efferent activity in the sympathetic nerves supplying
the adrenal, spleen, and interscapular brown adipose tissue after the
above administrations of aFGF. Both intravenous and
intracerebroventricular administration of 10 ng basic FGF (bFGF) also
increased sympathetic adrenal efferent activity and plasma Epi and NE
concentrations. However, the increases induced by 10 ng bFGF were
smaller than those induced by 10 ng aFGF. Bilateral splanchnicotomy
completely prevented the increases in Epi induced by
intracerebroventricular or intravenous aFGF but had less effect on the
increases in NE. Pretreatment with an antibody against corticotropin-releasing factor (CRF), given via the
intracerebroventricular route, significantly attenuated the increases
in Epi and NE evoked by intracerebroventricular or intravenous
administration of aFGF. Hepatic vagotomy also greatly reduced the
increases in both catecholamines and the increases in sympathetic
efferent firing rates evoked by intravenous administration of aFGF.
These findings indicate that 1) aFGF
administered intracerebroventricularly activates adrenomedullary
secretion and sympathetic outflow via CRF release and
2) aFGF injected intravenously also
induces sympathoadrenomedullary activation via centrally released CRF.
The idea is discussed that sympathetic activation induced either by
endogenous aFGF after feeding or by exogenously administered aFGF may
play roles both in energy expenditure after overeating and in the
modulation of immune functions.
sympathetic activity; corticotropin-releasing factor; energy
expenditure; overfeeding; autoimmune function
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INTRODUCTION |
ACIDIC AND BASIC fibroblast growth factors (aFGF and
bFGF), which influence the proliferation and differentiation of various cell types in vitro, were originally isolated as single chain proteins
from neural tissue, including whole brain and hypothalamus (3).
Recently, it has become clear from a number of studies that FGFs have a
wide spectrum of effects on neurophysiological activities that are
distinct from their mitogenic action within the central nervous system
(CNS) in vivo. For instance, when administered into the brain, aFGF
protects against the degeneration of hippocampal CA1 neurons that is
induced by brain ischemia (28). Endogenous aFGF enhances
learning and memory processes and facilitates long-term potentiation in
hippocampal CA1 neurons (16, 25, 27). Endogenous aFGF and bFGF are
released from the ependymal cells of the cerebral third ventricle into
the cerebrospinal fluid (CSF) after food intake (8, 29) and act as feed
suppressants via the inhibition of glucose-sensitive neurons in the
lateral hypothalamic area (LHA) (8, 15, 25, 29). Furthermore,
intracisternal injection of bFGF both suppresses secretion of gastric
acid and reduces the severity of experimentally induced gastric mucosal
lesions in rats (23). Interestingly, aFGF exhibits ~55% sequence
identity with the basic type and the two forms interact with the same
cell-surface receptors (20). However, the suppressant action of aFGF on
feeding is about twofold stronger than that of bFGF (8), whereas aFGF but not bFGF induces both thermogenesis, leading to a <1°C
increase in body temperature, and non-rapid eye movement (REM) sleep
(14).
It is well known that corticotropin-releasing factor (CRF) mediates
activation of the hypothalamo-sympatho-adrenomedullary axis (5) as well
as of the hypothalamic-pituitary-adrenal axis and that CRF is closely
associated with anorexia in humans (9) and rats (1). In addition, it
has been shown that a microinjection of CRF into the ventromedial
hypothalamus (VMH) diminishes the gastric mucosal damage induced by
cold restraint (7). Furthermore, by its central action, an acute
application of CRF facilitates the process of memory formation (17).
Moreover, glucocorticoid is linked to long-term potentiation in CA1
neurons in the hippocampus (11). These observations led us to
hypothesize that FGFs exogenously administered may lead to activation
of the hypothalamo-sympatho-adrenomedullary system via a release of CRF
in the brain. This idea is consistent with the fact that exogenous and
endogenous aFGF both induce reactions similar to the integrated
physiological responses induced by CRF. Indeed, we have reported that
when administered centrally exogenous aFGF potentiates the
hypothalamic-pituitary-adrenal axis via CRF release (18). Thus the
purpose of this study was to investigate whether and how
1) aFGF activates sympathetic
efferent activity, 2) aFGF increases
plasma catecholamines, and 3) CRF in
the brain is linked to the increase in catecholamines.
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MATERIALS AND METHODS |
Animals and surgery. Male Wistar rats
weighing 350-400 g, housed individually with a 12:12-h light-dark
cycle, were maintained at a room temperature of 24 ± 1°C with
free access to food and water. All procedures were approved by the
Animal Care and Use Committee of Nagasaki University and conformed to
guidelines for the use of laboratory animals published by the Japanese
government (law no. 105, Oct. 1, 1973). For intracerebroventricular
infusion, a guide cannula made of 23-gauge stainless steel tubing was
fixed into the cerebral third ventricle 2 wk before the experiments. Three days before the experiments, a chronically indwelling silicone catheter was implanted into the atrium through the right jugular vein
and brought out subcutaneously at the back of the neck. To measure mean
arterial blood pressure (MAP) and heart rate (HR), a polyethylene
catheter (OD 0.8 mm, ID 0.4 mm) was placed into the aorta via the
femoral artery and a silicone catheter was implanted into the right
atrium via the right jugular vein (both in 28 animals). These catheters
were brought out subcutaneously at the back of the neck. When required,
the arterial catheter could be connected to a strain gauge pressure
transducer (Nihon Kohden PT300T) for the recording of MAP and HR.
Animals were allowed 3 days to recover from the surgery before any
measurements were taken. Three weeks before the experiments, the
splanchnic nerves were dissected bilaterally below the diaphragm (SPX)
in 14 rats and the hepatic branch of the vagus nerve (arising from the
right side of the left general vagus nerve) was sectioned in 9 rats (HVX). All surgical procedures were performed under
pentobarbital sodium anesthesia (50 mg/kg ip).
Experimental protocol. On the day of
the experiment, each animal was anesthetized with pentobarbital sodium
(25 mg/kg iv) via the implanted catheter. The depth of anesthesia was
maintained by giving additional injections of pentobarbital sodium (7.5 mg/kg iv) every 30 min, starting 1 h after the first dose. A 29-gauge stainless steel tube connected to a polyethylene tube filled with test
solution was inserted into the guide cannula. The 29-gauge tube was
adjusted so that its tip was level with the tip of the guide cannula.
Then, aFGF dissolved in artificial cerebrospinal fluid (aCSF)
containing 0.1% bovine albumin was infused at a rate of 2 µl/min
over a period of 1-5 min. For intravenous administration, aFGF was
dissolved in saline containing 0.1% bovine albumin and infused over a
period of 1-2 min. For control experiments, equal amounts of aCSF
containing 0.1% bovine albumin or saline containing 0.1% bovine
albumin were used as the injectant. Heat-inactivated aFGF (90°C, 15 min) at the highest dose used in each series of experiments was also
employed as an additional control. In experiments with anti-CRF
antibody, the interval between its intracerebroventricular infusion and
the intracerebroventricular or intravenous infusion of aFGF was ~20
min. Doses of aFGF by a given route were applied in a randomized order.
Through the implanted venous catheter, 0.4-ml blood samples were slowly
drawn, as required, each over a 2-min period 10 min before and 20, 40, 60, 90, 120, 150, and 180 min after an administration of drug or
vehicle. Blood cells resuspended in the same volume of saline after
centrifugation were slowly returned to the animal within 2 min of the
end of every blood-sampling episode (except the first). After the first sampling, 0.4 ml saline was given as replacement. MAP and HR were recorded on a polygraph system (Nihon Kohden AP620-G) throughout the
experiment, and values were measured during 15 s just before and 15 s
just after each withdrawal of blood or replacement of resuspended blood
cells (which was done in exactly the same way as the blood sampling for
the determination of plasma catecholamines). All experimental
procedures involving blood sampling were performed between 0900 and
1400. Plasma samples were stored at 
80°C with 0.2% EDTA for
<2 mo until assayed for catecholamines. Activity in sympathetic
efferent and vagal afferent nerves was recorded using the method
reported previously (21, 22). In brief, animals were anesthetized with
-chloralose (65 mg/kg) plus urethan (0.8 g/kg) after food
deprivation for 6 h. Under a dissecting microscope, nerve filaments
were isolated from the central cut end of the left adrenal or splenic
branch of the splanchnic nerve and from a nerve serving the
interscapular brown adipose tissue (BAT). These were used to provide
recording of sympathetic efferent outflow. To observe afferent signals,
nerve filaments were isolated from the peripheral cut end of the
hepatic branch of the vagus nerve. The nerve filaments so isolated were
covered with a mixture of liquid paraffin and white Vaseline. Efferent
or afferent discharges recorded from fine filaments of the nerves
through a pair of silver wire electrodes were amplified and displayed
on an oscilloscope, recorded on a pen recorder, and stored on magnetic
tape. All such activity was analyzed after conversion of raw data to
standard pulses with the aid of a window discriminator that separated
discharges from background noise. A ratemeter with a reset time of 5 s
was used to enable us to follow the time course of the nerve activity. The nerve activity was analyzed by comparing the mean frequency per
5 s over 50-s periods at various times before and after
administration of aFGF and by comparing the activity induced by drugs
with that recorded after vehicle administration.
Administration of drugs. aFGF and bFGF
(R&D Systems) were dissolved in 10 µl aCSF containing 0.1% bovine
albumin. Lyophilized anti-CRF antibody (Peptide Institute; containing
50 µl rabbit antiserum against human CRF) was dissolved in 50 µl
aCSF. When required, 10 µl of this anti-CRF antibody solution
(containing 10 µl antiserum) was administered
intracerebroventricularly to an animal 20 min before the start of the
experiment.
Measurements. Plasma catecholamines
were measured by the coulometric electrochemical determination method,
with the minor modification previously reported (19). The minimum
detectable concentration of the catecholamines under study was within
the range of 3-5 pg/vial. Integrated catecholamine responses (area under the curve) were also calculated after administration of aFGF or
vehicle. The integrated responses reported here represent the increment
above basal level over a 180-min period after each application.
Statistical analysis. Data were
analyzed by a one- or two-way ANOVA, with a correction for repeated
measures, by means of a computer software program designed for
statistical analysis (Fisher, Tokyo University, Tokyo, Japan), as
reported elsewhere (19). When a significant overall effect was revealed
by ANOVA, the significance of differences from the prestimulus value
within a given group and between groups at each time point was tested by appropriate post hoc statistics using the same computer software system.
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RESULTS |
Effects of intracerebroventricular administration of
aFGF on plasma Epi and NE. An intracerebroventricular
administration of 1 or 10 ng/rat aFGF induced dose-dependent increases
in the plasma levels of both Epi and NE (Fig.
1, A and
B). A significant increase in Epi
was first detected at 60 min, and the response seemed to be peaking at
150 min. At 180 min after the aFGF administration (when sampling
ended), it was showing no sign of returning to the basal level. Similar
changes were observed in plasma NE levels. Injection of heat-treated
aFGF (10 ng) induced no such increases in plasma catecholamines. The
integrated responses (over the 180 min after aFGF administration) also
showed dose-dependent increases in Epi and NE (Fig. 1,
A and
B,
insets). In absolute terms, the integrated Epi response was more than two times the NE response at each
dose of aFGF.
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Fig. 1.
Effect of intracerebroventricular acidic fibroblast growth factor
(aFGF) on plasma epinephrine (Epi) and norepinephrine (NE)
concentrations. A: plasma Epi before
and after administration of heat-inactivated 10 ng icv aFGF
(n = 8) or aFGF at 1 (n = 7) or 10 ng icv/rat
(n = 10).
Inset: integrated Epi response (over
180 min after intracerebroventricular administration).
B: plasma NE before and after
administration of heat-inactivated 10 ng icv aFGF
(n = 8) or aFGF at 1 (n = 7) or 10 ng icv/rat
(n = 10).
Inset: integrated NE response (over
180 min after intracerebroventricular administration).
n, Number of animals. Values are means ± SE.  P < 0.05, P < 0.01 vs.
heat-inactivated aFGF control at same time point.
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Effects of intravenous administration of aFGF on
plasma Epi and NE. Dose-dependent increases in plasma
Epi and NE were also observed in response to 1, 10, and 100 ng aFGF
given intravenously (Fig. 2,
A and
B). The plasma Epi level showed a
gradual and long-lasting increase and reached a plateau at or before
180 min when 1 or 10 ng aFGF was administered, but, when 100 ng aFGF
was administered, the level was still rising at 180 min. Significant
increases in NE were evoked from 60 to 120 min or more after
intravenous administration of 10 or 100 ng aFGF. Heat-treated aFGF (100 ng) had no effect on the level in plasma catecholamines. The integrated
responses also showed dose-dependent increases in plasma Epi and NE
when aFGF was injected intravenously (Fig. 2,
A and
B,
insets). In absolute terms, the
integrated Epi and NE responses to 100 ng aFGF given via the
intravenous route were almost the same size as those induced by
one-tenth of the dose (i.e., 10 ng aFGF) administered via the
intracerebroventricular route.
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Fig. 2.
Effect of intravenous aFGF on plasma Epi and NE concentrations.
A: plasma Epi before and after
administration of heat-inactivated 100 ng iv aFGF
(n = 8) or of aFGF at 1 (n = 5), 10 (n = 7), or 100 ng iv/rat
(n = 5).
Inset: integrated Epi response (over
180 min after intravenous administration).
B: plasma NE before and after
administration of heat-inactivated 100 ng iv aFGF
(n = 8) or aFGF at 1 (n = 5), 10 (n = 7), or 100 ng iv/rat
(n = 5).
Inset: integrated NE response (over
180 min after intravenous administration). Values are means ± SE.
P < 0.05, P < 0.01 vs.
heat-inactivated control at same time point.
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Effects of intracerebroventricularly or intravenously
administered aFGF on MAP and HR. MAP showed a gradual
increase with a peak at ~60 min after an intracerebroventricular
administration of 10 ng aFGF. MAP was significantly higher at 60 (132 ± 5.3 mmHg), 90 (134 ± 6.3 mmHg), and 120 (130 ± 9.2 mmHg)
min after aFGF administration than at the same times after vehicle
injection (Fig.
3A,
bottom). In animals given aFGF
intracerebroventricularly, HR ranged between 320 and 354 beats/min
throughout the study period, whereas in vehicle control animals it was
between 310 and 344 beats/min. There was no significant difference
between the two groups (Fig. 3A,
top). MAP decreased immediately
after blood sampling by 3.18 ± 0.98 and 2.40 ± 0.83 mmHg in
vehicle- and aFGF-injected groups, respectively (Fig.
3A,
inset). After the replacement of
blood cells resuspended in saline, MAP increased by 2.25 ± 0.57 and 2.30 ± 0.81 mmHg in vehicle- and aFGF-injected groups, respectively (Fig. 3A,
inset). In terms of the changes in
MAP (
MAP) associated with blood sampling (withdrawal) or blood
replacement (replacement) no significant difference was found between
aFGF- or vehicle-injected animals (Fig.
3A,
inset). When aFGF or vehicle was
administered via the intravenous route, no significant changes in MAP
or HR were observed throughout the experimental period (Fig.
3B). Again, MAP decreased
immediately after blood sampling, this time by 4.88 ± 1.63 and 3.90 ± 1.40 mmHg, in vehicle- and aFGF-injected groups, respectively
(Fig. 3B,
inset). After the replacement of
resuspended blood cells, MAP increased by 5.25 ± 1.43 and 3.98 ± 1.40 mmHg in vehicle- and aFGF-injected groups, respectively
(Fig. 3B,
inset). In terms of the changes in
MAP associated with blood withdrawal or replacement, no significant
difference was found between aFGF- and vehicle-injected animals (Fig.
3B,
inset).
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Fig. 3.
Effect of aFGF on heart rate (HR) and mean arterial blood pressure
(MAP). A: HR
(top) and MAP
(bottom) before and after
administration of 10 ng icv/rat aFGF
(n = 6) or vehicle
(n = 8).
Inset: mean MAP (difference between
MAP before and after blood withdrawal or before and after blood
replacement) in animals given aFGF or vehicle
intracerebroventricularly. B: HR
(top) and MAP
(bottom) before and after
intravenous administration of aFGF (n = 6) or vehicle (n = 8).
Inset: mean MAP in animals given
aFGF or vehicle intravenously. Values are means ± SE.
# P < 0.05 vs. vehicle control
at same time point.
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Effects of aFGF on sympathetic efferent discharge to
the adrenal gland. In response to 10 ng icv aFGF, the
sympathetic efferent activity in the adrenal nerve showed a clear
increase (in terms of the multiunit discharge rate) starting at ~15
min and reaching significance at or before 30 min (Fig.
4A). The
mean discharge rate showed a dose-dependent increase, and the increases
induced by 1 or 10 ng/rat aFGF were both significantly greater than
that induced by vehicle (Fig. 4A,
inset). When administered
intravenously, 10 ng/rat aFGF again markedly facilitated the discharge
(Fig. 4B). By comparison with the
basal level, the mean discharge rate at 90 min after the 10 ng/rat
administration was increased by ~86% (intracerebroventricularly) or
67% (intravenously) (see Fig. 4, A
and B,
insets). Administration of vehicle
by the intracerebroventricular or intravenous route caused no
detectable change in nerve activity.
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Fig. 4.
Effect of intracerebroventricular or intravenous administration of aFGF
on the efferent firing rate in a sympathetic branch of the left adrenal
nerve. A: efferent discharge rate in
response to vehicle (bottom) or aFGF
at 1 (middle) or 10 ng icv
(top).
Inset: mean discharge rates (±SE)
for vehicle (n = 3) and for 1 (n = 10) and 10 ng icv
(n = 10) aFGF
intracerebroventricularly. B: efferent
discharge rate in response to vehicle
(bottom) or aFGF at 10 ng iv
(top).
Inset: mean discharge rates (±SE)
for vehicle (n = 3) and 10 ng iv aFGF
(n = 10).
# P < 0.05. ## P < 0.01 vs. vehicle control at same time point.
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Effects of aFGF on sympathetic efferent discharge to
the spleen and BAT. In the splenic efferent nerves, a
significant facilitation of the discharge rate was evoked by an
intracerebroventricular administration of 10 ng aFGF, the response
beginning at ~38 min and continuing for >180 min (Fig.
5A,
top). When 10 ng aFGF was administered via the intravenous route, the discharge rate at first
gradually decreased, reaching a minimum level at 30 min, but thereafter
gradually increased and showed a significant potentiation from 100 min
up to at least 210 min (Fig. 5A,
bottom). In response to 10 ng iv
aFGF, the discharge rate in the sympathetic efferent nerves to BAT
decreased slightly, but not significantly, until ~30 min and then
increased markedly up to ~120 min (Fig.
5B). By comparison with vehicle
control, the mean discharge rate was significantly increased at 60 (28% above the basal level ), 90 (33%), and 120 (37%) min after the
intravenous administration of aFGF (Fig.
5B,
inset). No detectable change in
nerve activity to the spleen or BAT was found after an administration
of vehicle by the intravenous route.
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Fig. 5.
Effect of intracerebroventricular or intravenous aFGF on efferent
firing rate in sympathetic branches supplying the spleen
(A) or left interscapular brown
adipose tissue (BAT; B).
A: records of firing rate before and
after intracerebroventricular (top)
or intravenous (bottom)
administration of 10 ng aFGF. B:
records of firing rate before and after injection of 10 ng iv aFGF
(top) or vehicle
(bottom).
Inset: mean discharge rates (±SE)
for aFGF (n = 10) and vehicle
(n = 3).
# P < 0.05 vs. vehicle control
at same time point.
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Effects of bFGF on sympathetic efferent discharge to
the adrenal gland. In response to 10 ng icv bFGF, the
sympathetic efferent activity in the adrenal nerve showed a clear
increase at 20 min after the injection, and it reached a plateau level
around 90 min. The mean discharge rate increased from 30 to 120 min
after the administration of 10 ng icv bFGF (much as it did after 10 ng
icv aFGF) (Fig. 6,
A and
B). Thereafter, it gradually
decreased to the basal level. The mean discharge rate at 210 min was
~23% lower with bFGF than with aFGF (Fig.
6A). When administered
intravenously, bFGF again significantly facilitated the sympathetic
efferent activity in the adrenal nerve at 60 min after the injection
(Fig. 6, A and
C). A comparison with the effect on
the mean discharge rate induced by the same dose of aFGF showed that
although the response induced by intravenous bFGF reached comparable
levels to those induced by aFGF at 180 and 210 min after its
administration, the mean discharge rates at 60, 90, 120, and 150 min
after bFGF administration were, respectively, 19, 16, 14, and 11%
lower than those recorded after induced intravenous aFGF (Fig.
6A). Administration of vehicle by
the intracerebroventricular or intravenous route caused no detectable
change in nerve activity (Fig. 6, B
and C).
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Fig. 6.
Effects of basic FGF (bFGF) on the efferent firing rate in a
sympathetic branch supplying the adrenal gland.
A: mean discharge rates (±SE) for
10 ng aFGF given intracerebroventricularly
(n = 10) or intravenously
(n = 10), for 10 ng bFGF given
intracerebroventricularly (n = 6) or
intravenously (n = 6), and for vehicle
intracerebroventricularly (n = 5) or
intravenously (n = 5).
# P < 0.05 vs. vehicle control
at same time point. B: efferent
discharge rates in response to 10 ng icv/rat bFGF
(top) or vehicle
(bottom).
C: efferent discharge rates in
response to 10 ng iv/rat bFGF (top)
or vehicle (bottom).
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Effects of intracerebroventricular or intravenous
administration of bFGF on plasma Epi and NE. An
intracerebroventricular or intravenous administration of 10 ng/rat bFGF
also increased the plasma levels of Epi (Fig.
7A) and
NE (Fig. 7B). After an intracerebroventricular injection, a significant increase in Epi was
first detected at 60 min. The Epi response peaked at 120 min after aFGF
administration and then showed a downward trend. After intravenous
administration of 10 ng bFGF, small but significant increases in Epi
levels were observed at 40 and 60 min. The integrated responses also
showed significant increases in Epi in animals given both
intracerebroventricular and intravenous administrations (Fig.
7A,
inset). In absolute terms, the
integrated Epi response induced by 10 ng icv bFGF was ~32% of that
induced by 10 ng icv aFGF, whereas that induced by 10 ng iv bFGF was
22% of the integrated response induced by 10 ng iv aFGF. The plasma NE
concentration also showed small but significant increases, and it
reached a plateau at 90 min when 10 ng bFGF was administered
intracerebroventricularly. After intravenous administration of 10 ng
bFGF, small but significant increases in NE were detected at 90 and 120 min. Small but significant increases were also observed in the
integrated NE responses in animals given both intracerebroventricular
and intravenous administration (Fig.
7B,
inset). In absolute terms, the
integrated NE response to 10 ng icv bFGF was about one-half that
induced by 10 ng aFGF. When bFGF was given via the intravenous route,
the integrated NE response to 10 ng bFGF was 60% of that seen in
response to 10 ng aFGF. Thus the effects of bFGF on adrenomedullary
secretion and sympathetic efferent activity to the adrenal gland were
both considerably weaker than those of aFGF.
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Fig. 7.
Effect of intracerebroventricular or intravenous bFGF on plasma Epi and
NE concentrations. A: plasma Epi
before and after administration of vehicle
(n = 8) or 10 ng icv/rat bFGF
(n = 7) and before and after
administration of vehicle (n = 9) or
10 ng iv/rat bFGF (n = 8).
Inset: integrated Epi responses to 10 ng bFGF or aFGF given either intracerebroventricularly
(left) or intravenously
(right). Responses were integrated
over 180 min after administration. B:
plasma NE before and after administration of vehicle
(n = 8) or 10 ng icv/rat bFGF
(n = 7) and before and after
administration of vehicle (n = 9) or 10 ng iv/rat bFGF (n = 8).
Inset: integrated NE responses to 10 ng/rat bFGF or aFGF given either intracerebroventricularly
(left) or intravenously
(right). Responses were integrated
over the 180 min after administration. Values are means ± SE.
# P < 0.05 vs. vehicle,
$ P < 0.05 vs. 10 ng aFGF.
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Effects of aFGF on afferent activity in the hepatic
vagus nerve. Afferent activity in the hepatic branch of
the vagus increased dose dependently when doses of 10, 50, and 100 ng
aFGF were given over 1-min periods into the portal vein (ipv) (Fig.
8A).
Administration of vehicle by the portal vein route did not cause any
significant change in nerve activity (not shown). Significant increases
in activity could be seen at ~10 min after the start of the
injections. After 10 or 50 ng aFGF, the response peaked at ~26 min
and the firing rate then gradually decreased toward the basal level.
When 100 ng aFGF was administered, the increase was extremely long lasting; it had not yet reached a maximal level at 120 min after the
injection.
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Fig. 8.
Effect of portal vein administration (ipv) of aFGF on afferent firing
rate in the hepatic branch of the left vagus nerve
(A) and effect of hepatic vagotomy
(HVX) on the increase in efferent firing rate of sympathetic branches
supplying the spleen (B;
top) or adrenal gland
(B;
bottom). Responses in
B were evoked by aFGF given
intravenously (top) or into the
portal vein (bottom).
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Effects of HVX on the aFGF-evoked increases in
sympathetic outflow and plasma Epi and NE. HVX
completely prevented the increases in efferent activity in the
sympathetic nerves innervating the spleen and adrenal that were evoked
in intact animals by administration of aFGF (20 ng iv and 100 ng ipv,
respectively) (Fig. 8B). The increases in plasma Epi and NE concentrations evoked by intravenous aFGF were markedly reduced in HVX rats at 90, 120, 150, and 180 min
after the injection (Fig. 9,
A and
B). The integrated increases in
plasma Epi and NE induced by intravenous administration of 10 ng aFGF
were also greatly reduced in HVX rats (36.9 and 44.3%, respectively,
of the response seen in intact animals) (Fig. 9, A and
B,
inset).
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Fig. 9.
Effect of pretreatment with anti-corticotropin-releasing factor (CRF)
antibody (by intracerebroventricular application), bilateral
splanchnicotomy (SPX), and HVX on the increases in plasma Epi and NE
concentration induced by intravenous aFGF.
A: plasma Epi before and after
administration of 10 ng iv aFGF in intact animals with
(n = 10) or without
(n = 7) anti-CRF antibody, in animals
without anti-CRF after either SPX (n = 8) or HVX (n = 9), and in intact
animals given an injection of heat-inactivated 100 ng iv aFGF
(n = 8).
Inset: integrated Epi response
(integrated over the 180 min after aFGF administration) induced by 10 ng iv aFGF under the above conditions.
B: plasma NE before and after
administration of 10 ng iv aFGF in intact animals with
(n = 10) or without
(n = 7) anti-CRF antibody, in animals
without anti-CRF after either SPX
(n = 8) or HVX
(n = 9), and in intact animals given
an injection of heat-inactivated 100 ng iv aFGF
(n = 8).
Inset: integrated NE response
(integrated over 180 min after aFGF administration) induced by 10 ng iv
aFGF under the above conditions. Values are means ± SE.
P < 0.01 vs.
heat-inactivated aFGF in intact animals.
# P < 0.05, ## P < 0.01 vs. aFGF
administered without anti-CRF antibody pretreatment in intact
animals.
|
|
Effects of anti-CRF antibody or SPX on the aFGF-evoked
increases in Epi and NE. The basal levels of plasma Epi
and NE were not changed significantly by pretreatment with anti-CRF
antibody (via the intracerebroventricular route). However, such
pretreatment strongly attenuated the aFGF-induced increases in Epi and
NE at 90, 120, 150, and 180 min after the injection (Figs.
10, A
and B). The integrated increases in
both Epi and NE were reduced to about one-third of the responses seen
in animals without such pretreatment (Fig. 10,
A and
B,
insets). Furthermore, in animals given 10 ng aFGF by the intravenous route, pretreatment with anti-CRF antibody significantly lowered the plasma levels of Epi and NE evoked
by aFGF (Fig. 9, A and
B). This effect could be clearly seen by examining the integrated increases in Epi and NE, which showed
reductions of 64 and 70.4%, respectively, after anti-CRF antibody treatment (Fig. 9, A and
B, insets). Bilateral SPX
completely prevented the increases in plasma Epi concentration
seen in intact animals after the intravenous (Fig.
9A) or intracerebroventricular (Fig.
10A) administration of 10 ng aFGF.
In fact, the integrated increases in Epi when aFGF was given by the
intravenous route (Fig. 9A,
inset) or the
intracerebroventricular route (Fig.
10A, inset) in splanchnicotomized rats
were ~10 and 6%, respectively, of the responses seen in intact
animals; they thus became comparable to the responses to
heat-inactivated aFGF seen in intact animals. Although the plasma NE
response was significantly reduced by splanchnicotomy at 90, 120, 150, and 180 min when aFGF was administered intracerebroventricularly (Fig.
10B), it was unchanged by the same
maneuver when aFGF was administered intravenously (Fig.
9B). In fact, the integrated increase in NE induced by the intracerebroventricular application of
aFGF was attenuated by ~54% in SPX animals, but that induced by its
intravenous application was reduced by only ~18%, not significantly (Figs. 9B and
10B,
insets). Thus SPX affected the
aFGF-induced increases in Epi much more than the increases in NE.
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Fig. 10.
Effect of pretreatment with anti-CRF antibody (by
intracerebroventricular application) and bilateral SPX on the increases
in plasma Epi and NE concentration induced by intracerebroventricular
aFGF. A: plasma Epi before and after
administration of 10 ng icv/rat aFGF in intact animals with
(n = 6) or without
(n = 10) anti-CRF antibody treatment,
in animals without anti-CRF antibody treatment after SPX
(n = 6), and in intact animals given
heat-inactivated 10 ng aFGF (n = 8).
Inset: effect of the above treatments
on the increases in the integrated Epi response induced by 10 ng icv
aFGF (integrated over 180 min after aFGF administration).
B: plasma NE before and after
administration of 10 ng icv aFGF in intact animals with
(n = 6) or without
(n = 10) anti-CRF antibody treatment,
in animals without anti-CRF antibody treatment after SPX
(n = 6), and in intact animals given
heat-inactivated 10 ng aFGF (n = 8).
Inset: effect of the above treatments
on the increases in the integrated NE response induced by 10 ng icv
aFGF (integrated over 180 min after aFGF administration). Values are
means ± SE. P < 0.01 vs. heat-inactivated aFGF in intact animals.
# P < 0.05, ## P < 0.01 vs. aFGF
administered without anti-CRF antibody pretreatment in intact
animals.
|
|
| |
DISCUSSION |
In this study, it was shown that not only exogenous aFGF but also
exogenous bFGF induced activations of sympathetic outflow and
adrenomedullary secretion, although aFGF was more effective than bFGF.
This observation is consistent with our previous finding that aFGF has
a suppressant effect on feeding behavior that is about twofold stronger
than that of bFGF (8) and with the observation reported by Knefati et.
al. (14) that aFGF, but not bFGF, has somnogenic and thermogenic
actions. In the present study, heat treatment completely abolished the
effects otherwise induced by aFGF. Although after blood withdrawal MAP
decreased by 3.18 ± 0.98 and 4.88 ± 1.63 mmHg, after blood
replacement it increased again by 2.25 ± 0.57 and 5.25 ± 1.43 mmHg (in animals given aFGF via the
intracerebroventricular and intravenous routes, respectively). In
vehicle-injected animals, the changes in MAP after blood sampling or
replacement were comparable to those seen in aFGF-injected animals. In
fact, there were no statistical differences among the decreases in MAP
or among the increases whether rats were given vehicle,
intracerebroventricular aFGF, or intravenous aFGF. A long-lasting
activation of the sympathetic efferent nerves innervating the adrenal,
spleen, and BAT accompanied the increase in MAP observed in animals
given aFGF intracerebroventricularly, but not in vehicle-injected animals. Thus it is unlikely that these increases in sympathetic efferent activity and in plasma catecholamines were secondary to any
changes in MAP associated with blood sampling and/or
replacement. The activation of sympathetic outflow and the increased
adrenomedullary secretion induced by aFGF seem to be specific responses
to aFGF itself.
aFGF administered intracerebroventricularly induced dose-dependent
increases not only in the plasma levels of Epi and NE but also in the
efferent firing rate in the sympathetic adrenal nerves in our
anesthetized rats. Doses of 1 and 10 ng icv would give final
concentrations in the CSF of ~0.2 and 2.1 pmol/ml (CSF volume: 300 µl). These concentrations are within the physiological range, because
the basal aFGF level in the CSF is 0.7 pmol/ml and the level increased
to 0.7 nmol/ml at 15 min and 7.5 nmol/ml at 45 min after food intake or
after 4 mM icv glucose application (8, 25). The most important results
in the present intracerebroventricular experiments were as follows. The
increases in plasma Epi and adrenal efferent nerve activity persisted
for up to 180 min after an intracerebroventricular application of aFGF.
The integrated Epi response induced by 10 ng icv aFGF was some 2.5 times greater than the corresponding NE response. Bilateral SPX
completely abolished the increase in Epi but not the increase in NE. On
the other hand, pretreatment with anti-CRF antibody via the
intracerebroventricular route significantly attenuated not only the
increases in Epi evoked by 10 ng aFGF via the intracerebroventricular
and intravenous routes but also the increases in NE. In fact, the
integrated increases in Epi and NE were both reduced to ~30% of
those seen in the intact animal.
On intravenous administration of aFGF, marked and long-lasting
increases in Epi and NE were again observed, together with increases in
adrenal sympathetic efferent activity. The injected aFGF doses of 1, 10, and 100 ng would give final plasma concentrations of 6.3, 63, and
630 fmol/ml if the rat's plasma volume is assumed to be 11 ml on
average. These are also within the physiological range. When given
intravenously, aFGF caused a facilitation of sympathetic efferent
activity not only to the adrenal gland but also to the spleen and BAT.
The integrated Epi response was ~3.4 times the corresponding NE
response. In this study, aFGF was significantly less potent when
injected intravenously than when injected centrally in both evoking
increases in the integrated Epi and NE responses (67% and 48.3%,
respectively, of the responses to intracerebroventricular aFGF) and
facilitating the efferent activity in the sympathetic adrenal nerves
(82.3% of the intracerebroventricular response at 90 min after the
injection). The effects of SPX on the integrated increases in Epi and
NE were different: the former were completely abolished, whereas the
latter were reduced by one-half or less (the response to intravenous
aFGF being affected much less than that to intracerebroventricular
aFGF). Pretreatment with anti-CRF antibody, which attenuated the
increases in Epi and NE by 62 and 68%, respectively, when aFGF was
administered centrally, attenuated them by 71 and 68% when aFGF was
given peripherally. HVX abolished almost completely not only the
integrated increases in Epi and NE but also the intravenous
aFGF-induced potentiation of the sympathetic efferent outflow to the
adrenal, spleen, and BAT. Recently, we reported that
microelectrophoretic application of aFGF to parvocellular neurons of
the PVN in vitro increased neuronal activity in more than one-third of
the neurons tested (30). It may be that aFGF administered centrally
potentiates the sympathoadrenomedullary axis via an activation of
parvocellular CRF neurons.
Interestingly, marked increases in the plasma corticosterone level have
been found after intravenous or intracerebroventricular administration
of aFGF (18). However, pretreatment with an intracerebroventricular injection of anti-CRF antibody reduced the integrated increases in
corticosterone by ~60% when aFGF was administered centrally but by
only 25% (not significantly) when it was administered peripherally (18). In the same study, peripheral aFGF application activated the
pituitary and provoked ACTH release (18) and HVX did not affect the
corticosterone increase when aFGF was administered peripherally. These
observations and the present ones indicate that
1) the activation of the
sympathoadrenomedullary axis by peripherally administered aFGF occurs
in a quite different way from the activation of the
hypothalamic-pituitary-adrenal axis, and
2) when aFGF is administered
systemically, hepatic afferent impulses lead to increased CRF release
in the brain. Ultimately, the released CRF would lead to activation of
the sympathetic outflow and increases in Epi and NE via the
intermediolateral column, the origin of the efferent sympathetic
motoneurons. Possibly, hepatic afferent signals may be conveyed into
the nucleus of the solitary tract (NTS) and the neuronal input from the
NTS to the PVN may then trigger CRF release. In any event, centrally
released CRF after intravenous or intracerebroventricular
administration of aFGF seems likely to play a key role in the
activation of the hypothalamo-sympatho-adrenomedullary axis.
It is well known 1) that food intake
increases both sympathetic outflow (2, 13, 32) and urinary
catecholamine excretion (6, 12) and
2) that feeding or glucose ingestion
increases thermogenesis through an activation of BAT (22, 26, 32). In
the present study, aFGF induced parallel increases in the sympathetic efferent activity to the adrenal and BAT. In general, the firing rate
of the adrenal sympathetic efferent nerves is reciprocally related to
the blood glucose level (4, 21). By comparison with the response in
BAT, an inverse response was found in the adrenal efferent nerve
activity within 30 min after an intravenous injection of 300 mg/kg
glucose (21, 22). Thus whether the increases in urinary catecholamine
excretion and thermogenesis after feeding or glucose ingestion are
mediated by aFGF-induced adrenomedullary activation remains unknown.
The parallel activation of the sympathetic outflow to the adrenal and
BAT may show that aFGF has a multifunctional role in the control of
neuronal and/or endocrinological activity. Indeed, Knefati at.
al. (14) suggested that aFGF forms part of a complex cytokine network
in the brain, because intracerebroventricular aFGF but not bFGF induces
non-REM sleep and fever in rabbits (14). Intravenous administration of
aFGF (100 ng/rat) also induces a long-lasting hyperthermia of
<1°C in awake and freely moving rats (our unpublished
observation). These results suggest that the long-lasting fever induced
by exogenous aFGF given via the intravenous or intracerebroventricular
route is caused, at least in part, by activation of sympathetic nerves innervating the adrenal medulla and BAT via the release of CRF in the
brain.
Perspectives
A further area of interest is the link between aFGF and the immune
system. In the present study, exogenous aFGF activated the sympathetic
outflow to the spleen and adrenal medulla, and it also activates the
hypothalamic-pituitary-adrenal axis (18). Splenic natural killer cell
cytotoxicity is reduced by activation of the splenic sympathetic
outflow (with associated increases in plasma NE concentration), which
is in turn evoked via CRF release in the rat brain (10, 31).
Furthermore, it has become clear that catecholamines, as well as
glucocorticoids, should be viewed as physiological inhibitors of
inflammatory responses and as immunosuppressive mediators (33). These
data suggest that aFGF would be expected to affect the immune system.
Indeed, exogenous aFGF application protects against degeneration of
hippocampal CA1 neurons after experimental brain ischemia (28)
and attenuates the impairment of immune functions otherwise seen in
aged senescence-accelerated P8 mice (24).
| |
ACKNOWLEDGEMENTS |
We thank Dr. R. Timms for help in preparing the manuscript.
| |
FOOTNOTES |
This work was partly supported by the Japanese Ministry of Education,
Science, and Culture Grants-in-Aid 06454151, 09470015 (to K. Sasaki),
and 05558095 (Y. Oomura), and by the Science and Technology Agency by
way of Special Coordination funds for promoting Science and Technology
in Japan (to Y. Oomura and K. Sasaki)
Address for reprint requests: I. Matsumoto, Dept. of Physiology,
Nagasaki University School of Medicine, Nagasaki 852, Japan.
Received 23 June 1997; accepted in final form 24 June 1998.
| |
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Abstract
Introduction
