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NADPH-Diaphorase activity in neurons of the mammalian pancreas: Coexpression with vasoactive intestinal polypeptide
1993;105:999-1008
GASTROENTEROLOGY
NADPH-Diaphorase Activity in Neurons of the Mammalian Pancreas: Coexpression With Vasoactive Intestinal Polypeptide TOORU SHIMOSEGAWA, TAKASHI ABE, AKIHIKO MASARU KOIZUMI, and TAKAYOSHI TOYOTA Third Department
icotinamide
adenine
dinucleotide
phosphate-
diaphorase (NADPH-d) is an enzyme that catalyzes the chemical reaction of converting soluble ni-
troblue tetrazolium salt to insoluble blue dye formazan in the presence of NADPH.’ By histochemistry for NADPH-d, a specific group of neurons in the brain have been shown to possess the activity of this enzyme, although
REISHI
ABE,
YOSHIFUMI
KIKUCHI,
of Internal Medicine, Tohoku University School of Medicine, Sendai, Japan
Background: To provide a morphological basis for understanding the role of nitric oxide in the pancreas, the present study was designed to clarify the localization and distribution of nicotinamide adenine dinucleotide phosphate-diaphorase (NADPH-d) activity, a marker of NO synthase, in the pancreas of several mammalian species, including humans. Methods: NADPH-d activity was examined in the rat, guinea pig, dog, and human pancreas by histochemistry. In addition, the possibility of coproduction of NO and vasoactive intestinal polypeptide (VIP) was investigated by a combined use of histochemistry and immunohistochemistry. Results: In the pancreas, NADPH-d activity was localized in nerve fibers, nerve cell bodies, and the vascular endothelium. Nerve fibers with the enzyme activity were chiefly distributed in the exocrine pancreas and showed species differences in the distribution. Nerve fibers stained for NADPH-d were also observed in the endocrine pancreas, but the enzyme activity was not detected in the islet cells. Part of the nerve fibers and nerve cell bodies coexpressed NADPH-d activity and VIP-immunoreactivity. _Conclusions: These results suggest that NO may act as a neuronal mediator and an endothelium-derived relaxing factor and may physiologically interact with VIP in the mammalian pancreas.
N
SATOH,
its role has remained
unknown.’
Recently,
however, strong evidence has been presented that NADPH-d corresponds to neuronal nitric oxide synthase (NOS), which forms nitric oxide by conversion of L-arginine to L-citrulline.3-5 NO is a free radical gas, recently identified as an endothelium-derived relaxing factor,6s7 and may be a candidate for nonadrenergic, noncholinergic neurotransmitters in both the central and peripheral nerves.*-” It- is well known that pancreatic functions are under
the strong influence of autonomic nerves.” Besides the classical neurotransmitters like acetylcholine and noradrenaline, garded
various
small
peptides
as neurotransmitters
pancreatic ported
nerve
systems.13
that NADPH-d
detected result
in intrinsic
strongly
However,
activity, neurons
suggests
pancreatic
study,
and distribution because
of
we recently
a marker
re-
of NOS, was
of the rat pancreas.14
This
to classi-
neurotransmitters, should neuronal mediator regu-
we compared
of NADPH-d pigs,
dogs,
the colocalization
intestinal
re-
functions.
In the present of rats, guinea
been
that NO, in addition
cal and putative peptidergic be considered as a putative lating
have
or neuromodulators
the localization
activity and
humans.
of NOS-like
polypeptide-like
in the pancreas In addition, and vasoactive
immunoreactivity
(VIP-
LI) has recently been shown in guinea pig enteric neurons, l5 the possibility of coexpression was examined in the intrapancreatic
neurons.
Materials and Methods Materials ley rats (200-250
Pancreatic
specimens from five male Sprague-Dawg body wt), five male Hartley guinea pigs
(250-300
wt),
g body
five male
body wt), and five humans Two
fresh
from
the
operations, autopsy
specimens segments
Necropsy
patients
specimens
All pancreatic tine histological ducted
of human of resected
and three pancreatic
from
mongrel
dogs
(lo-15
were used in the present pancreas materials specimens
were
obtained
during
surgical
were obtained
who died of nonpancreatic were fixed within
specimens
with the consent
3 hours
The present
of the Ethics
at
diseases. after death.
were judged to be normal
examinations.
kg
study.
by rou-
study was con-
Committee
for Use of
Experimental Animals and Research Use of Human rials of the Tohoku University School of Medicine.
Mate-
Abbreviations used in this paper: NADPH-d, nicotinamide adenine dinucleotide phosphate-diaphorase; NOS, nitric oxide synthase; PFA, paraformaldehyde solution; VIP-L& vasoactive intestinal polypeptide-like immunoreactivity. Q 1993 by the American Gastroenterological Association 0016-5085/93/$3.00
1000
GASTROENTEROLOGY Vol. 105. No. 4
SHIMOSEGAWA ET AL.
Figure 1. NADPH-d actmty in the pancreas. (A)Nerve fibers around acini in the human pancreas (original magnification x500). (8) Nerve fibers around intralobular ducts in the guinea pig pancreas (original magnification X485). (C) Nerve fibers around a capillary in the rat pancreas (original magnification x500). (D) Nerve plexus around a small artery in the rat pancreas (original magnification X410). (E) An interlobular nerve bundle containing numerous nerve fibers in the dog pancreas (original magnification X3 10). (F)Nerve fibers and terminals in an islet of the rat pancreas (original magnification x525).
Fixation and Tissue Preparation While under deep anesthesia with sodium pentobarbital (60 mg/kg Nembutal;
Tokyo-Kasei,
Tokyo, Japan),
rats and guinea pigs were perfused with 60 mL of ice-cold saline through the ascending aorta, followed by perfusion with 360 mL of ice-cold (PFA)
in phosphate
2% paraformaldehyde
solution
buffer (pH 7.4, 0.1 mol/L)
solution.
The pancreas was quickly removed and divided into the head, body, and tail segments. The tissue pieces were then immersed in 2% PFA for 12-24
hours at 4°C. Dogs were
laparotomized under deep anesthesia with sodium pentobarbital (60 mg/kg), and specimens were excised from the head, body, and tail segment of the pancreas. The tissue pieces were immersed in cold 2% PFA for at least 48 hours at 4°C. Specimens of the human pancreas were quickly immersed in cold 2% PFA and kept there for at least 48 hours at 4°C. After fixation, all pancreatic specimens were kept in cold phosphate-buffered saline (PBS; pH 7.2, 0.01 mol/L) containing 10% sucrose for 24 hours at 4°C for cryoprotection. Tissue sections were cut to a thickness of 12 pm on a cryostat (Leitz 1720 digital cryostat; Ernst Leitz Wetzlar,
Table 1. Distribution of NADPH-d-Stained
Nerve Fibers in
the Pancreas Tissues
Rat
Exocrine pancreas Aclni Duct systems Large-caliber ducts Small-caliber ducts Vascular systems Capillaries Arterioles Arteries Venules Large-caliber veins Nerve fibers In nerve bundles Endocrine pancreas Islet. cells t. few; t+,
Guinea pig
Human
Dog
+++
++
+t
++ +
+ +++
++ +
+ ++
+ +++
+++ ++
++ +++
++ ++
t
+
+
+
+
+
t
+
++
+
+
+
t-t+
mixture
reflected
light
455 were used as exciter
t+t+
dak Tri-X
-t
moderate; +++.
abundant;
+++t,
Germany).
All sections
VIP-Antiserum
alum gelatin-coated taining Osaka,
0.3%
by a method
VIP-L1
Japan)
X-100
at 4°C
until
(Wako
anti-VIP
+
A, calcitonin Y, porcine
(Oriental
Yeast
nitroblue (pH
Co. Ltd.,
tetrazolium
8) containing
stained
for VIP
glycerol
tissue
(Wako)
X-100
was stopped
sections
were
pus BHS microscope
Tris-HCl
by rinsing
buffer at
the sections
in
a mixture
of
with
examined
(Olympus
field
for 60 minutes
covered
and PBS (2:1, vol/vol),
P-NADPH
Optical
Co. Ltd.,
the indirect
immunofluorescence
the anti-VIP
serum
Inc., Belmont, 24 hours
7161N;
According
methionine
for 60 minutes
1:700 for the anti-VIP
secondary
antibody.
The
One hundred
the anti-VIP
substance
tissues
serum were
for
rat, guinea P, secretin,
somatostatin,
fourth
specimens
section
nerve
cell bodies
with
only VIP-L1 activity,
pancreas,
and
error of deviation)
cell body was calculated
cut
species. described (1)
activity,
(2)
(3) nerve
cell
and (4) nerve cell bodactivity.
pig, dog,
These percentof the rat, guinea
the mean
percentage
of the respective
in each animal
type
species.
Results
The dilutions 1: 160 for the in a PBS-
animal
activity,
for every specimen
of nerve
Within Nerve
and NADPH-d
and NADPH-d
human
photomi-
were determined:
ages were determined and
by
for VIP immu-
as previously
VIP-L1
+ standard
bright-
evaluated
were consecutively
was processed
with
(mean
Previously
under
of the four
cell bodies
Scientific Inc., Nasections in a moist
mounted
staining. was
of the following
VIP-L1
were
and the same
bright-field
nerve
activatingpolyG conjugated
and
locations
rephotographed
to 200 sections
all pancreatic
and
by the
stainings.
ies without
at room temperature.
used were
with
precise
Percentage of Colocalization Cell Bodies from
fibers
photographed removed,
the corresponding
for NADPH-d
bodies with only NADPH-d
with fluorescein isothiocyanate (Miles perville, IL) was applied to the tissue
and
first immuno-
photomicrographs
chamber
27, glucagon,
pepto the
Nerve
Colocalization
Laboratories
endothelin-1, and pituitary adenylatecyclase peptide 38. Goat anti-rabbit immunoglobulin
chamber
by
were
the dark-field with
were
for NADPH-d
fields
in a moist
with
releasing
P, neu-
of VIP-LI.
were
and their
Peninsula
with porcine,
VIP, but none
histidine
Incubation
to the supplier,
100% cross-reactivity
pig, and human peptide
method.
CA) was performed
at 4°C.
serum shows
(RAS
was performed
VIP-L1
were then
nostainings crographs
Every for VIP
gastrin
described.
microscope,
and the percentages
lmmunohistochemistry
porcine
sections
The coverslips visual
comparing
Tokyo,
lmmunohistochemistry
with
illumination.3s4
using an Olym-
Japan) with a green filter, and photographed with Fuji Neopan F-film (lso 32; Fuji Photo Film Co., Tokyo, Japan).
tissue
were processed
recorded
and 0.2 mmol/L
in 0.1 mol/L
peptide,
of NADPH-d Activity
as previously
cell bodies
sections
by incubating
1 mmol/L Japan)
0.2% Triton
3i”‘C4 The reaction PBS. The
Tokyo,
porcine
of substance
or Met-enkephalin-Arg6-Gly’-Leu*
The pancreatic
Co.,
for histochemistry
was performed with
species exam-
of 100 pg/mL
galanin,
abol-
VIP to the
in PBS con-
recorded.
sections
of porcine
did not affect the strength
fluorescence
tissue
was completely
gene-related
Colocalization VIP-LI
Histochemistry slide--mounted
in tissues were per-
1:700) in any animal
the addition
bombesin,
nerve
staining
Ko-
Co., Roches-
reported.16
of the pancreas
serum (dilution,
ropeptide
and/Nor immunohistochemistry.
NADPH-d
Kodak
of VIP-L1
more than 0.2 pg/mL
ined. However,
tide,
Pharmaceutical
processed
filter.
with
Specificity
previously
in nerves
ished by adding
up on chrome
glass slides and immersed
Triton
and EY-
as a barrier
were photographed
Tests of the specificity formed
very dense.
were picked
filters, and O-515
sections
BHS-RFC
BP-490
ter, NY).
++t+
+
with an Olympus microscope.
pan film (Iso 400; Eastman
neurokinin +t+
and examined fluorescence
The immunostained
+
++
glycerol
antiserum
Wetzler,
1001
NADPH-D ACTIVITY IN THE PANCREAS
October 1993
tivity
Localization Activity
and Distribution
In all animal
species
shown
by blue-colored
of NADPH-d
examined,
NADPH-d
staining
was localized
acin
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SHIMOSEGAWA
ET AL.
GASTROENTEROLOGY
Vol. 105,
No. 4
NADPH-D ACTIVITY IN THE PANCREAS
October 1993
nerve
fibers,
thelium cies
nerve
cell bodies,
of the pancreas. differences
NADPH-d
in
activity
tween
body,
spe-
in nerve
of
rat and
In
within
they were not different
be-
and
distribution
neural
and tail segments
of the pan-
creas. NADPH-d
activity
the .parenchyma whereas
pancreas.
In the human
gicall specimens
than
In general, single dles with NADPH-d in the exocrine
pancreas,
in autopsy
nerve
fibers
observed
with in sur-
specimens.
close
to acini
guinea
showed
(Figure
2F and H).
that NADPH-d
staining
terminals
surrounded
(Figure
1E). NADPH-d
ure lF),
terminals
nerve bundistributed (Figure
lA),
but it was not detected
of any animal The density
species
pancreas,
slightly
man pancreas,
of NADPH-d
moderately
in
the islets (Fig-
in the endocrine positive
arteries
nerve
around
NADPH-d lium
density
in the walls
of thicker
ducts,
species activity
examined, were
fine nerve
fibers
acini
and
observed
moderate
whereas
with
moderately
or
in
in the
the enzyme abundantly
around arterioles, where they formed nerve plexuses. Species differences were remarkable in the innervation of islets; in the rat islets, many dotlike nerve terminals
pig and hu(Fig-
activity
veins (Fig-
of endothelial
and the individual staining
(Figure
was not detected or small
cells were 3B and C).
in the endothe-
veins.
C).
fibers
The
distribution
was essentially
However,
nerve
similar
of VIP-L1
to that
in the dog and human
of VIP-L1 nerve fibers that of NADPH-d-positive In the rat, guinea
appeared nerve
animal
much fibers.
that
higher
pancreas,
than
many of ganstrong
VIP (Figure 2A, C, and G). pancreas, most nerve cell bodimmunoreactivity for VIP (Figviews, VIP-L1 within perikarya
in the appearance.
surrounded
species.
the density
the nerve cell bodies within the intrapancreatic glia showed weak to moderate and occasionally
nals
nerve
of NADPH-d-
pancreas
pig, and human
was granular was
pattern
fibers of the respective
in the periphery
of the islets.
of VIP-LI in
As has been shown previously,‘“21 VIP-L1 was localized in nerve elements of the pancreas (Figure 4,4
with NADPH-d activity were observed, whereas in other animal species they were only occasionally seen activity
activity
and large-caliber
by strong
immunoreactivity for Meanwhile, in the dog ies showed very strong ure 2E). In magnified
Nerve cell bodies. NADPH-d
that
in the dog
of arterioles,
Localization and Distribution Pancreatic Nerves
in
they were present ducts. In all animal
fibers
in the guinea
The cytoplasm
pale blue,
of capillaries
positive
guinea pig and human pancreas, more densely around small caliber
activity
were dense
in the endothelium
3A andB),
bordered
rat and dog pancreas,
were
showed
and only sparse in the rat pancreas
(Figure
cells stained
and
fibers
views
and homogeneous
NADPH-d
less dense
also observed
capillaries of the guinea pig, dog, and human pancreas, whereas they were less dense in the rat pancreas. In the nerve
High-power
cells
animals is summarized in NADPH-d activity were
or abundantly
of this en-
Other tissue components. NADPH-d was
examined.
the pancreata of the various Table 1. Nerve fibers with observed
tissues
was also localized within
cell bodies
ure 2I3, D, F, and H).
connective
activity
fibers and nerve
nerve activity
was diffuse
cell bodies
clearly
nerve
most strong
with
ganglion
the
interlobular
of in-
in the perikarya.
ure 3C) in the pancreas.
and
terminals
2B, 13, F, and H). In the
pig pancreas,
around ducts (Figure lB), capillaries (Figure lC), arterioles and arteries (Figure lo), and in nerve bundles in intralobular
and nerve
(Figure
zyme (Figure 2B and D), whereas fewer nerve cell bodies stained for NADPH-d in the human and dog pan-
Nerve
in the rat
nerve trunks and thin activity were chiefly
pancreas
in
and human
less abundant
were more clearly
fibers
distributed
pig, dog,
they were
activity
of nerve
were diffusely
of the guinea
pancreas, NADPH-d
abundance
cell bodies
ganglia
the ganglia
creas
Nerve fibers. An with
shown
trapancreatic
elements.
density
however,
endo-
were considerable
in pancreatic
the same species, the head,
and the vascular
There
1003
nerve
Dotlike
cell bodies
nerve
termi-
also showed
Figure 2. Colocalizahon of NADPH-d actlvrty and VIP-L1 In intrapancreatic ganglion nerve cell bodies. Photomicrographs A. C, E, and G show VIP-LI, and B, D, F, and H show NADPH-d activity. (A and 8) Rat pancreas. All nerve cell bodies in this ganglion show both VIP-LI and NADPH-d activity (original magnification X390). (C and D) Guinea pig pancreas. Most nerve cell bodies in this ganglion show weak to moderate strength of VIP-L1 (C). and most show strong activity for NADPH-d (D) (original magnrfication x415). (E and F) Dog pancreas. Most nerve cell bodies show strong immunoreactivity for VIP (E), but only a few stain for NADPH-d (original magnification x390). (G and H) Human pancreas. Some nerve cell bodies show both VIP-LI and NADPH-d activity, but some show only VIP-L1 (original magnrfication x280).
1004
SHIMOSEGAWA ET AL.
GASTROENTEROLOGY Vol. 105, No. 4
for VIP.
immunoreactivity
nerve
terminals
within
The
density
of VIP-L1
intrapancreatic
ganglia
was
high in the guinea pig, dog, and human pancreas but low in the rat pancreas (Figure 2A, C, E, and G).
Colocalization VIP-LI Nerve fibers.
of NADPH-d Activity
In the rat and guinea pig pan-
creas, many nerve fibers around arterioles ducts showed
and
both VIP-L1
and small
and NADPH-d
activity
(Figure 4A and B), but some showed only VIP-L1 NADPH-d
activity.
In the dog and human pancreas,
numerous nerve fibers showed VIP-L& showed NADPH-d
or
but only a few
activity (Figure 4C and 0). VIP-L1 and NADPH-d
Nerve cell bodies. ity were also colocalized
activ-
in some of the nerve cell bod-
ies within the intrapancreatic
ganglia (Figure U-H).
In the rat and guinea pig pancreas, many of the nerve cell bodies
(Figure
2A-D)
NADPH-d
activity,
whereas in the human pancreas
coexpressed
slightly fewer did the same (Figure contrast,
in the dog pancreas,
VIP-L1
and
2G and H). By
most nerve cell bodies
showed VIP-L1 but only a small part of them simultaneously showed NADPH-d activity (Figure 2E and F). In the dog pancreas, it seemed that nerve cell bodies with a weak or negative
immunoreactivity
were stained strongly for NADPH-d
for VIP
(Figure 2E and
0 To determine which
VIP-L1
calized, 92-196
the percentage of nerve cell bodies in and NADPH-d intrapancreatic
ined in each specimen.
activity
were colo-
neurons
were exam-
The results are summarized in
Table 2. In the rat and guinea pig pancreas,
VIP-L1
and NADPH-d activities were colocalized in 86% and 78% of nerve cell bodies, respectively. In these animals, more than 80% of intrapancreatic ies showed VIP-L1 man
and
activities
Figure 3. NADPH-d activrty in the vascular endothelium of the pancreas. (A) Endothelium of an artery stained for NADPH-d in the human pancreas. The asterisk indicates the arterial lumen (original magnification X195). (6) Endothelial cells showing strong starning for NADPH-d in an artery of the guinea pig pancreas. The asterisk indicates the arterial lumen (original magnification X590). (C) A sheet of an endothelial layer of a large-caliber vein in the guinea prg pancreas. The cytoplasm of endothelial cells stains weakly for NADPH-d. and the individual cells are delineated by strong staining for NADPH-d (original magnification X350).
dog
or NADPH-d
pancreas,
were colocalized
VIP-L1
nerve cell bod-
activity. In the huand
NADPH-d
in 53% and only 16% of
nerve cell bodies, respectively. 80% and 75% of total nerve
However, more than cell bodies examined
showed VIP-L1 in the dog and human pancreas, respectively. No particular differences were noted in the strength of VIP-L1 or NADPH-d activity within the nerve cell bodies or in the percentage of nerve cell bodies with VIP-L1 and/or NADPH-d activity between surgical and autopsy specimens of the human pancreas. Nerve cell bodies that showed neither VIPLI nor NADPH-d activity were
October 1993
Figure 4. Colocalization of NADPH-d activity and VIP-L1 in nerve fibers of the pancreas. (A and 13)The same visual field of a section of the rat pancreas, immunostarned for VIP (A) and stained for NADPH-d (B). Most nerve fibers around an arteriole show both VIP-L1 and NADPH-d activity, but some show only one type of activity. The strong fluorescence in A is an artifact of staining (original magnification X660). (C and D) Nerve fibers around capillaries of the dog pancreas, immunostained for VIP (C) and stained for NADPH-d (D). Thin nerve bundles containing numerous VIP-LI nerve fibers surround capillaries, whereas only a few nerve fibers show NADPH-d activity. It is also noted that VIP-LI and NADPH-d activity are colocalized In some nerve fibers (original magnification x600).
Discussion
atic nerve
In this study, we showed that the presence of NADPH-d activity in neurons and vascular endothelium was a finding common to the rat, guinea pig, dog, and human colocalized
pancreas and that NADPH-d activity was with VIP-L1 within a part of intrapancre-
Table 2. Percentage of Nerve Cell Bodies With NADPH-d Activity and/or VIP-LI in the Pancreas Nerve cell type NADF’H-d+, NADPH-d-, NADF’H-d+, NADPH-d-,
VIP+ VIP+ VIPVIP-
Rat
Guinea pig
Dog
Human
86 + 2 a&i 61+1 0.2 i 0.2
78 t 4 a&2 a*3 3-+1
16 + 6 66 f 5 lOk3 a+ i
53 t 2 23? 1 19?2 3fl
NOTE. The numbers shown for each type of neuron are percentages (mean + SE) of the total nerve cell bodies examined. +, positive; -, negatrve.
fibers and nerve
cell bodies.
Recent
studies
have presented strong evidence that NADPH-d corresponds to neuronal NOS. 3,4 Our present histochemical results, together with the evidence, suggest that the nerves and vascular endothelium of the pancreas may produce NO, which may work as a neuronal mediator and an endothelium-derived relaxing factor in the mammalian pancreas. The presence of several isoforms of NOS has been clarified.22-24 By biochemical characteristics, these isoforms have been classified into two major categories. One is designated as the constitutive NOS, present in neurons and vascular endothelium, and the other as the inducible NOS, present in macrophages, neutrophils, pancreatic islet cells, or hepatocytes.23-25 Recent reports suggest that the constitutive NOS is localized in the rat islet cells or in the cultured rat insulinoma cells and that NO produced in islet cells may be the
1006
SHIMOSEGAWA
mediator
of arginine-stimulated
Careful tion
observations
activity
of guanylate of cyclic
cyclase
guanosine
and the resultant
the only known
numerous
activity
in the rat islets,
obtained
of other
cells agrees with but
NADPH-d
activity
previous
disagrees
cells.25*26 There
animal
activity
in
ancy, but the possibility
pancreatic
should
endocrine
as a neuronal
activity parenchyma,
activity
ganglion
cells,
re-
cells by the activation
of
and it has been
suggested
pancreatic
acinar
are increased
cells,
intracellular
by acetylcholine,
levels
providing in acinar
cells. 36-38 However,
ported
that elevation
(at least
troprusside
release.39 As shown and nerve in the
It is, therefore,
have
nerve from been
with
NADPH-d
vascular
by nitrosourea
on Ca2+ fluxes
the neurotransmitter
could be roughly
grouped
walls of the mouse.28
they suggested a general capable of producing NO
the intracellular
signal
into the enteric
and parasym-
pathetic postganglionic nerves. Our findings indicate that intrinsic neurons of the mammalian pancreas should also be added to the nerve systems that may produce NO. Nerve bundles
in intralobular
and interlobular
nective tissues of all animal species examined tained numerous nonvaricose nerve fibers NADPH-d activity, suggesting that extrapancreatic
con-
neurons
rat and guinea were
coexpressed
pig pancreas, coexpressed
or neuromo-
transduction
by NO and the biological pancreas.
and VIP-LI, suggesting that these duce both NO and VIP as neuronal VIP-L1
nerve fibers not only in
it is important action
pancreatic
is localized in nerve cell bodies pharynx, bladder walls, pelvic
or ni-
or amylase
study, were distributed
role of NO in the pancreas,
induced exocrine
re-
but also in ducts and acini in the pan-
creas. To establish clarify
it has been
in the p resent
activity
systems
dulator
of cGMP
has no effect
NADPH-d activity within the tongue,
and the intestinal
bom-
cyclase
The present study of colocalization and nerve cell bodies confirmed that
Based on these observations, rule that peripheral neurons
of cGMP
cholecystokinin,
regarded as the parasympathetic postganglionic. Recently, it has been shown by Grozdanovic et al. that
nerve plexuses,
that gua-
nylate cyclase-dependent mechanisms are involved in the insulin secretion from islet B cells.35 In dispersed
phore,
were diffusely
which
path-
that NO
endocrine
conceivable that at least a part of intrapancreatic fibers stained for NADPH-d may have originated the intrapancreatic
muscle
confirmed
and A231 87, a calcium ionoproof of the presence of guanylate
were shown
examined.
cyclase
signal transduction
are
physalaemin,
mediator.
in the pancreatic
guanylate
smooth
produc-
(cGMP)
besin,
the pancreatic
fibers with NADPH-d
of all the animals
on rat
laxes arterial
intracellular
No. 4
showing
be considered
that NO regulates
cell bodies with NADPH-d
Our
for this discrep-
in the rat pancreas) functions
species.
in pancreatic
others
is no clear explanation
ob-
was not
observations
with rat
termi-
were
this finding
of no NADPH-d
pancreas2’
nerve
for NADPH-d
although
in the pancreas
observation
dotlike
Vol. 105,
monophosphate
way for NO. 30-34 It has been
a strong
pancreas
tion
species
with
Nerve
vation
but no
nals
within
the localiza-
islet cells,
By contrast,
distributed
secretion.25’26
was seen in the islet cells of any animal
examined. served
insulin
were made to clarify
of NADPH-d
staining
acinar
GASTROENTEROLOGY
ET AL.
to
pathway
of NO on the in nerve fibers a part of intra-
NADPH-d
activity
neurons may promediators. In the
NADPH-d in a large
activity
and
proportion
of
nerve cell bodies within the ganglia (about 80%). However, in the dog and human pancreas, only about 16% and 53% of ganglion cell bodies, respectively, coexpressed them, although in both animal species more than 75% of nerve cell bodies showed VIP-LI. These observations strongly suggest that VIP-containing rons in the mammalian pancreas could be divided
neuinto
conwith ori-
two groups: neurons capable of synthesizing both VIP and NO and neurons synthesizing only VIP. Most
gins with the enzyme activity may also contribute to the innervation of the pancreas. In rats, NADPH-d activity has been shown in the nerve cell bodies of the sensory ganglia,‘” but not in the nerve cell bodies of the sympathetic ganglia. ‘* It is possible, therefore, that nerve fibers with sensory origins may constitute a part of the NO-synthesizing nerve system in the mammalian pancreas. Species differences were evident in the distribution of NADPH-d-positive nerve fibers in the pancreas, suggesting that NO may exert different modes of action on the pancreas from species to species. The acti-
nerve cell bodies in the rat and guinea pig pancreas correspond with the first type, whereas in the dogpancress, the latter type neurons are dominant. Because the variation of the ratio of the two types of VIP neurons was relatively small in the respective animal species, the ratio may be genetically determined from species to species. The importance of VIP in the mammalian pancreas was suggested by the presence of VIP-L1 in most neurons in the pancreas, irrespective of animal species. Meanwhile, the existence of NADPH-d activity in only a part of VIP-L1 neurons in the dog pancreas suggests that NO may exert a supple-
October 1993
ment-ary
NADPH-D ACTIVITY IN THE PANCREAS
role for VIP or may bear some specialized
in the pancreas of at least the dog species. By immunohistochemistry, it has been that
NADPH-d
choline
is colocalized
acetyltransferase
in certain
in the brain.40T4’ Recently, LI and VIP-L1
has been
teric neurons,15
mdicating
sion and coproduction to th.e intrinsic but instead
systems
needed
to
meaning
neurons
clarify
suggested
neuropeptide groups
of neurons
the colocalization shown
Y or
of NOS-
in the guinea
that the possible
pig encoexpres-
of NO and VIP are not specific
represent
nervous
with
role
of the mammalian a general
of digestive
pancreas,
rule for the intrinsic
organs.
the
physiological
of the possible
coproduction
Further
study
and
biological
is
fiber types innervating the taenia of the guinea-pig caecum. Cell Tissue Res 1992;270: 125- 137. 16. ShimosegawaT, Moriizumi S, Koizumi M, Kashimura J, Yanaihara N, Toyota T. lmmunohistochemical demonstration of galaninlike immunoreactive nerves in the human pancreas. Gastroenterology 1992; 102~263-27 1. 17. Larsson LI. Innervation of the pancreas by substance P. enkephalin. vasoactive intestinal polypeptide and gastrin/CCK immunoreactive nerves. J Histochem Cytochem 1979;27: 1283- 1284. 18. Bishop AE, Polak JM, Green IC, Bryant MG, Bloom SR. The location of VIP in the pancreas of man and rat. Diabetologia 1980; 18:73-78. 19. DeGiorgio R, Sternini C, Anderson K, Brecha N, Go VLW. Tissue distribution and innervation pattern of peptide immunoreactivities in the rat pancreas. Peptides 1992;13:91-98. 20.
of NO and VIP.
References 1. Thomas E, Pearse AGE. The fine localization of dehydrogenases in the nervous system. Histochemie 196 1;2:266-282. 2. Scherer-Singler U, Vincent SR, Kimura H. McGeer EG. Demonstration of a unique population of neurons with NADPH-diaphorase histochemistry. J Neurosci Methods 1983;9:229-234. 3. Hope BT, Michael GJ, Knigge KM, Vincent SR. Neuronal NADPH diaphorase is a nitric oxide synthase. Proc Natl Acad SCI USA 199 1;88:28 1 1-28 14. 4. Dawson TM, Bredt DS, Fotuhi M, Hwang PM, Snyder SH. Nitnc oxide synthase and neuronal NADPH diaphorase are identical in brain and peripheral tissues. Proc Natl Acad Sci USA 1991;88:7797-7801. 5. Ward SM. Xue C, Shuttleworth CW, Bredt DS, Snyder SH, Sanders KM. NADPH diaphorase and mtric oxide synthase colocalizatlon in entenc neurons of canine proximal colon. Am J Physisol 1992;263:G277-G284. 6. Furchgott RF, Zawadzki JV. The obligatory role of endothelial cells in the relaxation of arterial smooth muscle by acetylcholine. Nature 1980;288:373-376. 7. Palmer RMJ, Ferrige AG, Moncada S. Nitric oxide release accounts for the biological activity of endothelium-derived relaxing factor. Nature 1987;327:524-526. 8. Snyder SH, Bredt DS. Nitric oxide as a neuronal messenger. Trends Pharmacol Sci 199 1; 12: 125- 128. 9. 13redt DS. Snyder SH. Nitric oxide, a novel neuronal messenger. Neuron 1992;8:3- 1 1. 10. !Sanders KM, Ward SM. Nitric oxide as a mediator of nonadrenergic noncholinergic neurotransmission. Am J Physiol 1992;262: G379-G392. 11. 13urnett AL, Lowenstein CJ, Bredt DS, Chang TSK, Snyder SH. INItric oxide: a physiologic mediator of penile erection. Science 1992;257:40 l-403. 12. Ilolst JJ. Neural regulation of pancreatic exocrine function. In: Go ‘VLW, Gardner JD, Brooks FP, Lebenthal E, DiMagno EP, Sheele GA, eds. The exocrine pancreas: biology, pathobiology, and disleases. New York: Raven, 1986:287-300. 13. Rauner BB. Handbook of physiology. Section 6: the gastrointestinal system. Volume II. Neural and endocrine biology. Bethesda, Maryland: American Physiological Society, 1989. 14. Shimosegawa T, Abe T, Satoh A, Asakura T, Yoshida K. Koizumi M, Toyota T. Histochemical demonstration of NADPH-diaphorase activity, a marker for nitric oxide synthase, In neurons of the rat pancreas. Neuroscl Lett 1992;148:67-70. 15. Furness JB. Pompolo S, Shuttleworth CWR, Burleigh DE. Lightand electron-microscopic immunochemical analysis of nerve
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DeGiorgio R, Sternini C, Brecha NC, Widdison AL, Karanjia ND, Reber HA, Go VLW. Patterns of innervation of vasoactive intestinal polypeptide, neuropeptide Y, and gastrin-releasing peptide immunoreactive nerves in the feline pancreas. Pancreas 1992;7:376-384.
21. Sundler F, Alumets J, H%kanson R, Fahrenkrug J, Schaffalitzky de Muckadell 0. Peptidergic (VIP) nerves in the pancreas. Histochemistry 1978;55: 173- 176. 22.
Bredt DS, Snyder SH. Isolation of nitric oxide synthetase, a calmodulin-requiring enzyme. Proc Natl Acad Sci USA 1990; 87~682-685.
23. Yui Y, Hattori R, Kosuga K, Eizawa H, Hiki K. Kawai C. Purification of nitric oxide synthase from rat macrophages. J Biol Chem 199 1;266: 12544- 12547. 24.
Xie QW, Cho HJ, Calaycay J, Mumford RA, Swiderek KM, Lee TD, Ding A, Troso T, Nathan C. Cloning and characterization of inducible nitric oxide synthase from mouse macrophages. Science 1992;256:225-228.
25.
Schmidt HHHW, Warner TD, lshii K, Sheng H. Murad F. Insulin secretion from pancreatic B cells caused by L-arginine-derived nitrogen oxides. Science 1992;255:721-723.
26. Schmidt HHHW, Gagne GD, Nakane M, Pollock JS, Miller MF, Murad F. Mapping of neural nitric oxide synthase in the rat suggests frequent co-localization with NADPH diaphorase but not with soluble guanylyl cyclase, and novel paraneural functions for nitrinergic signal transduction. J Histochem Cytochem 1992; 40: 1439- 1456. 27.
Vincent SR. Nitric oxide and arginine-evoked Science 1992;258: 1376.
insulin secretion.
28.
Grozdanovic Z, Baumgarten HG, Broning G. Histochemistty of NADPH-diaphorase, a marker for neuronal nitric oxide synthase. in the peripheral autonomic nervous system of the mouse. Neuroscience 1992;48:225-235.
29.
Aimi Y, Fujimura M, Vincent SR, Kimura H. Localization of NADPH-diaphorase-containing neurons in sensory ganglia of the rat. J Comp Neurol 1991;306:382-392.
30.
Rapoport RM, Murad F. Agonist induced endothelium-dependent relaxation in rat thoracic aorta may be mediated through cyclic GMP. Circ Res 1983;52:352-357.
Craven PA, DeRubertis FR. Restoration of the responsiveness of purified guanylate cyclase to nitrosoguanidine, nitric oxide, and related activators by heme and hemeproteins: evidence for involvement of the paramagnetic nitrosylheme complex in enzyme activation. J Biol Chem 1978;253:8433-8443. 32. Garthwaite J, Charles SL, Chess-Williams R. Endothelium-derived relaxing factor release on activation of NMDA receptors suggests role as intercellular messenger in the brain. Nature 1988;336:385-388. 33. Knowles RG, Palacios M, Palmer RMJ. Moncada S. Formation of nitric oxide from L-arginine in the central nervous system: a trans-
31.
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SHIMOSEGAWA ET AL.
ductron mechanism for stimulation of the soluble guanylate cyclase. Proc Nat1 Acad Sci USA 1989;86:5 159-5 162. 34.
Bredt DS, Snyder SH. Nitric oxide mediates glutamate-linked enhancement of cGMP levels in the cerebellum. Proc Natl Acad SCI USA 1989;86:9030-9033.
35.
Laychock SG. Evidence for guanosine 3’,5’-monophosphate as a putative mediator of insulin secretion from isolated rat islets. Endocrinology 198 1; 108: 1 197- 1205.
36. Christophe JP, Frandsen EK, Conlon TP, Krishna G, Gardner JD. Action of cholecystokinin, cholinergtc agents and A23187 on accumulabon of guanosine-3’,5’-monophosphate in dispersed guinea prg pancreatic acinar cells. J Biol Chem 1976;25 1:46404645. 37.
May RJ, Conlon TP, Erspamer V, Gardner JD. Actions of peptides isolated from amphibian skin on pancreatic acinar cells. Am J Physiol 1978;235:E 1 12-E 1 18.
38.
Uhlemann ER, Rottman AJ, Gardner JD. Actions of peptides ISOlated from amphibian skin on amylase release from dispersed pancreatic acini. Am J Physiol 1979;236:E57 1-E576.
39. Gunther GR. Jamieson JD. Increased
intracellular
cyclic GMP
does not correlate with protein discharge from pancreatic acmar cells. Nature 1979;280:318-320. 40. Armstrong DM, Saper CB, Levey Al, Wamer BH, Terry RD. Drstribution of cholinergic neurons in rat brain: demonstrated by the immunocytochemical localization of choline acetyltransferase. J Comp Neurol 1983;2 16:53-68. 4 1. Vincent SR, Johansson 0, Hokfelt T, Skirboll L, Elde RP, Terenrus L, Kimmel J, Goldstein M. NADPH-diaphorase: a selective histochemical marker for striatal neurons containing both somatostatm and avian pancreatic polypeptide (APP)-like immunoreactivities. J Comp Neurol 1983;2 17:252-263.
Received January 13, 1993. Accepted June 3, 1993. Address requests for reprints to: Tooru Shimosegawa, M.D., Third Department of Internal Medicine, Tohoku University School of Medicine, l-l Seiryo-machi, Aoba-ku, Sendai, Miyagi 980, Japan. The autopsy specimens of the human pancreas used in this study were supplied by the Department of Pathology and the surgical specimens by the First Department of Surgery, Tohoku University School of Medicine, Sendai, Japan.
GASTROENTEROLOGY
NADPH-Diaphorase Activity in Neurons of the Mammalian Pancreas: Coexpression With Vasoactive Intestinal Polypeptide TOORU SHIMOSEGAWA, TAKASHI ABE, AKIHIKO MASARU KOIZUMI, and TAKAYOSHI TOYOTA Third Department
icotinamide
adenine
dinucleotide
phosphate-
diaphorase (NADPH-d) is an enzyme that catalyzes the chemical reaction of converting soluble ni-
troblue tetrazolium salt to insoluble blue dye formazan in the presence of NADPH.’ By histochemistry for NADPH-d, a specific group of neurons in the brain have been shown to possess the activity of this enzyme, although
REISHI
ABE,
YOSHIFUMI
KIKUCHI,
of Internal Medicine, Tohoku University School of Medicine, Sendai, Japan
Background: To provide a morphological basis for understanding the role of nitric oxide in the pancreas, the present study was designed to clarify the localization and distribution of nicotinamide adenine dinucleotide phosphate-diaphorase (NADPH-d) activity, a marker of NO synthase, in the pancreas of several mammalian species, including humans. Methods: NADPH-d activity was examined in the rat, guinea pig, dog, and human pancreas by histochemistry. In addition, the possibility of coproduction of NO and vasoactive intestinal polypeptide (VIP) was investigated by a combined use of histochemistry and immunohistochemistry. Results: In the pancreas, NADPH-d activity was localized in nerve fibers, nerve cell bodies, and the vascular endothelium. Nerve fibers with the enzyme activity were chiefly distributed in the exocrine pancreas and showed species differences in the distribution. Nerve fibers stained for NADPH-d were also observed in the endocrine pancreas, but the enzyme activity was not detected in the islet cells. Part of the nerve fibers and nerve cell bodies coexpressed NADPH-d activity and VIP-immunoreactivity. _Conclusions: These results suggest that NO may act as a neuronal mediator and an endothelium-derived relaxing factor and may physiologically interact with VIP in the mammalian pancreas.
N
SATOH,
its role has remained
unknown.’
Recently,
however, strong evidence has been presented that NADPH-d corresponds to neuronal nitric oxide synthase (NOS), which forms nitric oxide by conversion of L-arginine to L-citrulline.3-5 NO is a free radical gas, recently identified as an endothelium-derived relaxing factor,6s7 and may be a candidate for nonadrenergic, noncholinergic neurotransmitters in both the central and peripheral nerves.*-” It- is well known that pancreatic functions are under
the strong influence of autonomic nerves.” Besides the classical neurotransmitters like acetylcholine and noradrenaline, garded
various
small
peptides
as neurotransmitters
pancreatic ported
nerve
systems.13
that NADPH-d
detected result
in intrinsic
strongly
However,
activity, neurons
suggests
pancreatic
study,
and distribution because
of
we recently
a marker
re-
of NOS, was
of the rat pancreas.14
This
to classi-
neurotransmitters, should neuronal mediator regu-
we compared
of NADPH-d pigs,
dogs,
the colocalization
intestinal
re-
functions.
In the present of rats, guinea
been
that NO, in addition
cal and putative peptidergic be considered as a putative lating
have
or neuromodulators
the localization
activity and
humans.
of NOS-like
polypeptide-like
in the pancreas In addition, and vasoactive
immunoreactivity
(VIP-
LI) has recently been shown in guinea pig enteric neurons, l5 the possibility of coexpression was examined in the intrapancreatic
neurons.
Materials and Methods Materials ley rats (200-250
Pancreatic
specimens from five male Sprague-Dawg body wt), five male Hartley guinea pigs
(250-300
wt),
g body
five male
body wt), and five humans Two
fresh
from
the
operations, autopsy
specimens segments
Necropsy
patients
specimens
All pancreatic tine histological ducted
of human of resected
and three pancreatic
from
mongrel
dogs
(lo-15
were used in the present pancreas materials specimens
were
obtained
during
surgical
were obtained
who died of nonpancreatic were fixed within
specimens
with the consent
3 hours
The present
of the Ethics
at
diseases. after death.
were judged to be normal
examinations.
kg
study.
by rou-
study was con-
Committee
for Use of
Experimental Animals and Research Use of Human rials of the Tohoku University School of Medicine.
Mate-
Abbreviations used in this paper: NADPH-d, nicotinamide adenine dinucleotide phosphate-diaphorase; NOS, nitric oxide synthase; PFA, paraformaldehyde solution; VIP-L& vasoactive intestinal polypeptide-like immunoreactivity. Q 1993 by the American Gastroenterological Association 0016-5085/93/$3.00
1000
GASTROENTEROLOGY Vol. 105. No. 4
SHIMOSEGAWA ET AL.
Figure 1. NADPH-d actmty in the pancreas. (A)Nerve fibers around acini in the human pancreas (original magnification x500). (8) Nerve fibers around intralobular ducts in the guinea pig pancreas (original magnification X485). (C) Nerve fibers around a capillary in the rat pancreas (original magnification x500). (D) Nerve plexus around a small artery in the rat pancreas (original magnification X410). (E) An interlobular nerve bundle containing numerous nerve fibers in the dog pancreas (original magnification X3 10). (F)Nerve fibers and terminals in an islet of the rat pancreas (original magnification x525).
Fixation and Tissue Preparation While under deep anesthesia with sodium pentobarbital (60 mg/kg Nembutal;
Tokyo-Kasei,
Tokyo, Japan),
rats and guinea pigs were perfused with 60 mL of ice-cold saline through the ascending aorta, followed by perfusion with 360 mL of ice-cold (PFA)
in phosphate
2% paraformaldehyde
solution
buffer (pH 7.4, 0.1 mol/L)
solution.
The pancreas was quickly removed and divided into the head, body, and tail segments. The tissue pieces were then immersed in 2% PFA for 12-24
hours at 4°C. Dogs were
laparotomized under deep anesthesia with sodium pentobarbital (60 mg/kg), and specimens were excised from the head, body, and tail segment of the pancreas. The tissue pieces were immersed in cold 2% PFA for at least 48 hours at 4°C. Specimens of the human pancreas were quickly immersed in cold 2% PFA and kept there for at least 48 hours at 4°C. After fixation, all pancreatic specimens were kept in cold phosphate-buffered saline (PBS; pH 7.2, 0.01 mol/L) containing 10% sucrose for 24 hours at 4°C for cryoprotection. Tissue sections were cut to a thickness of 12 pm on a cryostat (Leitz 1720 digital cryostat; Ernst Leitz Wetzlar,
Table 1. Distribution of NADPH-d-Stained
Nerve Fibers in
the Pancreas Tissues
Rat
Exocrine pancreas Aclni Duct systems Large-caliber ducts Small-caliber ducts Vascular systems Capillaries Arterioles Arteries Venules Large-caliber veins Nerve fibers In nerve bundles Endocrine pancreas Islet. cells t. few; t+,
Guinea pig
Human
Dog
+++
++
+t
++ +
+ +++
++ +
+ ++
+ +++
+++ ++
++ +++
++ ++
t
+
+
+
+
+
t
+
++
+
+
+
t-t+
mixture
reflected
light
455 were used as exciter
t+t+
dak Tri-X
-t
moderate; +++.
abundant;
+++t,
Germany).
All sections
VIP-Antiserum
alum gelatin-coated taining Osaka,
0.3%
by a method
VIP-L1
Japan)
X-100
at 4°C
until
(Wako
anti-VIP
+
A, calcitonin Y, porcine
(Oriental
Yeast
nitroblue (pH
Co. Ltd.,
tetrazolium
8) containing
stained
for VIP
glycerol
tissue
(Wako)
X-100
was stopped
sections
were
pus BHS microscope
Tris-HCl
by rinsing
buffer at
the sections
in
a mixture
of
with
examined
(Olympus
field
for 60 minutes
covered
and PBS (2:1, vol/vol),
P-NADPH
Optical
Co. Ltd.,
the indirect
immunofluorescence
the anti-VIP
serum
Inc., Belmont, 24 hours
7161N;
According
methionine
for 60 minutes
1:700 for the anti-VIP
secondary
antibody.
The
One hundred
the anti-VIP
substance
tissues
serum were
for
rat, guinea P, secretin,
somatostatin,
fourth
specimens
section
nerve
cell bodies
with
only VIP-L1 activity,
pancreas,
and
error of deviation)
cell body was calculated
cut
species. described (1)
activity,
(2)
(3) nerve
cell
and (4) nerve cell bodactivity.
pig, dog,
These percentof the rat, guinea
the mean
percentage
of the respective
in each animal
type
species.
Results
The dilutions 1: 160 for the in a PBS-
animal
activity,
for every specimen
of nerve
Within Nerve
and NADPH-d
and NADPH-d
human
photomi-
were determined:
ages were determined and
by
for VIP immu-
as previously
VIP-L1
+ standard
bright-
evaluated
were consecutively
was processed
with
(mean
Previously
under
of the four
cell bodies
Scientific Inc., Nasections in a moist
mounted
staining. was
of the following
VIP-L1
were
and the same
bright-field
nerve
activatingpolyG conjugated
and
locations
rephotographed
to 200 sections
all pancreatic
and
by the
stainings.
ies without
at room temperature.
used were
with
precise
Percentage of Colocalization Cell Bodies from
fibers
photographed removed,
the corresponding
for NADPH-d
bodies with only NADPH-d
with fluorescein isothiocyanate (Miles perville, IL) was applied to the tissue
and
first immuno-
photomicrographs
chamber
27, glucagon,
pepto the
Nerve
Colocalization
Laboratories
endothelin-1, and pituitary adenylatecyclase peptide 38. Goat anti-rabbit immunoglobulin
chamber
by
were
the dark-field with
were
for NADPH-d
fields
in a moist
with
releasing
P, neu-
of VIP-LI.
were
and their
Peninsula
with porcine,
VIP, but none
histidine
Incubation
to the supplier,
100% cross-reactivity
pig, and human peptide
method.
CA) was performed
at 4°C.
serum shows
(RAS
was performed
VIP-L1
were then
nostainings crographs
Every for VIP
gastrin
described.
microscope,
and the percentages
lmmunohistochemistry
porcine
sections
The coverslips visual
comparing
Tokyo,
lmmunohistochemistry
with
illumination.3s4
using an Olym-
Japan) with a green filter, and photographed with Fuji Neopan F-film (lso 32; Fuji Photo Film Co., Tokyo, Japan).
tissue
were processed
recorded
and 0.2 mmol/L
in 0.1 mol/L
peptide,
of NADPH-d Activity
as previously
cell bodies
sections
by incubating
1 mmol/L Japan)
0.2% Triton
3i”‘C4 The reaction PBS. The
Tokyo,
porcine
of substance
or Met-enkephalin-Arg6-Gly’-Leu*
The pancreatic
Co.,
for histochemistry
was performed with
species exam-
of 100 pg/mL
galanin,
abol-
VIP to the
in PBS con-
recorded.
sections
of porcine
did not affect the strength
fluorescence
tissue
was completely
gene-related
Colocalization VIP-LI
Histochemistry slide--mounted
in tissues were per-
1:700) in any animal
the addition
bombesin,
nerve
staining
Ko-
Co., Roches-
reported.16
of the pancreas
serum (dilution,
ropeptide
and/Nor immunohistochemistry.
NADPH-d
Kodak
of VIP-L1
more than 0.2 pg/mL
ined. However,
tide,
Pharmaceutical
processed
filter.
with
Specificity
previously
in nerves
ished by adding
up on chrome
glass slides and immersed
Triton
and EY-
as a barrier
were photographed
Tests of the specificity formed
very dense.
were picked
filters, and O-515
sections
BHS-RFC
BP-490
ter, NY).
++t+
+
with an Olympus microscope.
pan film (Iso 400; Eastman
neurokinin +t+
and examined fluorescence
The immunostained
+
++
glycerol
antiserum
Wetzler,
1001
NADPH-D ACTIVITY IN THE PANCREAS
October 1993
tivity
Localization Activity
and Distribution
In all animal
species
shown
by blue-colored
of NADPH-d
examined,
NADPH-d
staining
was localized
acin
1002
SHIMOSEGAWA
ET AL.
GASTROENTEROLOGY
Vol. 105,
No. 4
NADPH-D ACTIVITY IN THE PANCREAS
October 1993
nerve
fibers,
thelium cies
nerve
cell bodies,
of the pancreas. differences
NADPH-d
in
activity
tween
body,
spe-
in nerve
of
rat and
In
within
they were not different
be-
and
distribution
neural
and tail segments
of the pan-
creas. NADPH-d
activity
the .parenchyma whereas
pancreas.
In the human
gicall specimens
than
In general, single dles with NADPH-d in the exocrine
pancreas,
in autopsy
nerve
fibers
observed
with in sur-
specimens.
close
to acini
guinea
showed
(Figure
2F and H).
that NADPH-d
staining
terminals
surrounded
(Figure
1E). NADPH-d
ure lF),
terminals
nerve bundistributed (Figure
lA),
but it was not detected
of any animal The density
species
pancreas,
slightly
man pancreas,
of NADPH-d
moderately
in
the islets (Fig-
in the endocrine positive
arteries
nerve
around
NADPH-d lium
density
in the walls
of thicker
ducts,
species activity
examined, were
fine nerve
fibers
acini
and
observed
moderate
whereas
with
moderately
or
in
in the
the enzyme abundantly
around arterioles, where they formed nerve plexuses. Species differences were remarkable in the innervation of islets; in the rat islets, many dotlike nerve terminals
pig and hu(Fig-
activity
veins (Fig-
of endothelial
and the individual staining
(Figure
was not detected or small
cells were 3B and C).
in the endothe-
veins.
C).
fibers
The
distribution
was essentially
However,
nerve
similar
of VIP-L1
to that
in the dog and human
of VIP-L1 nerve fibers that of NADPH-d-positive In the rat, guinea
appeared nerve
animal
much fibers.
that
higher
pancreas,
than
many of ganstrong
VIP (Figure 2A, C, and G). pancreas, most nerve cell bodimmunoreactivity for VIP (Figviews, VIP-L1 within perikarya
in the appearance.
surrounded
species.
the density
the nerve cell bodies within the intrapancreatic glia showed weak to moderate and occasionally
nals
nerve
of NADPH-d-
pancreas
pig, and human
was granular was
pattern
fibers of the respective
in the periphery
of the islets.
of VIP-LI in
As has been shown previously,‘“21 VIP-L1 was localized in nerve elements of the pancreas (Figure 4,4
with NADPH-d activity were observed, whereas in other animal species they were only occasionally seen activity
activity
and large-caliber
by strong
immunoreactivity for Meanwhile, in the dog ies showed very strong ure 2E). In magnified
Nerve cell bodies. NADPH-d
that
in the dog
of arterioles,
Localization and Distribution Pancreatic Nerves
in
they were present ducts. In all animal
fibers
in the guinea
The cytoplasm
pale blue,
of capillaries
positive
guinea pig and human pancreas, more densely around small caliber
activity
were dense
in the endothelium
3A andB),
bordered
rat and dog pancreas,
were
showed
and only sparse in the rat pancreas
(Figure
cells stained
and
fibers
views
and homogeneous
NADPH-d
less dense
also observed
capillaries of the guinea pig, dog, and human pancreas, whereas they were less dense in the rat pancreas. In the nerve
High-power
cells
animals is summarized in NADPH-d activity were
or abundantly
of this en-
Other tissue components. NADPH-d was
examined.
the pancreata of the various Table 1. Nerve fibers with observed
tissues
was also localized within
cell bodies
ure 2I3, D, F, and H).
connective
activity
fibers and nerve
nerve activity
was diffuse
cell bodies
clearly
nerve
most strong
with
ganglion
the
interlobular
of in-
in the perikarya.
ure 3C) in the pancreas.
and
terminals
2B, 13, F, and H). In the
pig pancreas,
around ducts (Figure lB), capillaries (Figure lC), arterioles and arteries (Figure lo), and in nerve bundles in intralobular
and nerve
(Figure
zyme (Figure 2B and D), whereas fewer nerve cell bodies stained for NADPH-d in the human and dog pan-
Nerve
in the rat
nerve trunks and thin activity were chiefly
pancreas
in
and human
less abundant
were more clearly
fibers
distributed
pig, dog,
they were
activity
of nerve
were diffusely
of the guinea
pancreas, NADPH-d
abundance
cell bodies
ganglia
the ganglia
creas
Nerve fibers. An with
shown
trapancreatic
elements.
density
however,
endo-
were considerable
in pancreatic
the same species, the head,
and the vascular
There
1003
nerve
Dotlike
cell bodies
nerve
termi-
also showed
Figure 2. Colocalizahon of NADPH-d actlvrty and VIP-L1 In intrapancreatic ganglion nerve cell bodies. Photomicrographs A. C, E, and G show VIP-LI, and B, D, F, and H show NADPH-d activity. (A and 8) Rat pancreas. All nerve cell bodies in this ganglion show both VIP-LI and NADPH-d activity (original magnification X390). (C and D) Guinea pig pancreas. Most nerve cell bodies in this ganglion show weak to moderate strength of VIP-L1 (C). and most show strong activity for NADPH-d (D) (original magnrfication x415). (E and F) Dog pancreas. Most nerve cell bodies show strong immunoreactivity for VIP (E), but only a few stain for NADPH-d (original magnification x390). (G and H) Human pancreas. Some nerve cell bodies show both VIP-LI and NADPH-d activity, but some show only VIP-L1 (original magnrfication x280).
1004
SHIMOSEGAWA ET AL.
GASTROENTEROLOGY Vol. 105, No. 4
for VIP.
immunoreactivity
nerve
terminals
within
The
density
of VIP-L1
intrapancreatic
ganglia
was
high in the guinea pig, dog, and human pancreas but low in the rat pancreas (Figure 2A, C, E, and G).
Colocalization VIP-LI Nerve fibers.
of NADPH-d Activity
In the rat and guinea pig pan-
creas, many nerve fibers around arterioles ducts showed
and
both VIP-L1
and small
and NADPH-d
activity
(Figure 4A and B), but some showed only VIP-L1 NADPH-d
activity.
In the dog and human pancreas,
numerous nerve fibers showed VIP-L& showed NADPH-d
or
but only a few
activity (Figure 4C and 0). VIP-L1 and NADPH-d
Nerve cell bodies. ity were also colocalized
activ-
in some of the nerve cell bod-
ies within the intrapancreatic
ganglia (Figure U-H).
In the rat and guinea pig pancreas, many of the nerve cell bodies
(Figure
2A-D)
NADPH-d
activity,
whereas in the human pancreas
coexpressed
slightly fewer did the same (Figure contrast,
in the dog pancreas,
VIP-L1
and
2G and H). By
most nerve cell bodies
showed VIP-L1 but only a small part of them simultaneously showed NADPH-d activity (Figure 2E and F). In the dog pancreas, it seemed that nerve cell bodies with a weak or negative
immunoreactivity
were stained strongly for NADPH-d
for VIP
(Figure 2E and
0 To determine which
VIP-L1
calized, 92-196
the percentage of nerve cell bodies in and NADPH-d intrapancreatic
ined in each specimen.
activity
were colo-
neurons
were exam-
The results are summarized in
Table 2. In the rat and guinea pig pancreas,
VIP-L1
and NADPH-d activities were colocalized in 86% and 78% of nerve cell bodies, respectively. In these animals, more than 80% of intrapancreatic ies showed VIP-L1 man
and
activities
Figure 3. NADPH-d activrty in the vascular endothelium of the pancreas. (A) Endothelium of an artery stained for NADPH-d in the human pancreas. The asterisk indicates the arterial lumen (original magnification X195). (6) Endothelial cells showing strong starning for NADPH-d in an artery of the guinea pig pancreas. The asterisk indicates the arterial lumen (original magnification X590). (C) A sheet of an endothelial layer of a large-caliber vein in the guinea prg pancreas. The cytoplasm of endothelial cells stains weakly for NADPH-d. and the individual cells are delineated by strong staining for NADPH-d (original magnification X350).
dog
or NADPH-d
pancreas,
were colocalized
VIP-L1
nerve cell bod-
activity. In the huand
NADPH-d
in 53% and only 16% of
nerve cell bodies, respectively. 80% and 75% of total nerve
However, more than cell bodies examined
showed VIP-L1 in the dog and human pancreas, respectively. No particular differences were noted in the strength of VIP-L1 or NADPH-d activity within the nerve cell bodies or in the percentage of nerve cell bodies with VIP-L1 and/or NADPH-d activity between surgical and autopsy specimens of the human pancreas. Nerve cell bodies that showed neither VIPLI nor NADPH-d activity were
October 1993
Figure 4. Colocalization of NADPH-d activity and VIP-L1 in nerve fibers of the pancreas. (A and 13)The same visual field of a section of the rat pancreas, immunostarned for VIP (A) and stained for NADPH-d (B). Most nerve fibers around an arteriole show both VIP-L1 and NADPH-d activity, but some show only one type of activity. The strong fluorescence in A is an artifact of staining (original magnification X660). (C and D) Nerve fibers around capillaries of the dog pancreas, immunostained for VIP (C) and stained for NADPH-d (D). Thin nerve bundles containing numerous VIP-LI nerve fibers surround capillaries, whereas only a few nerve fibers show NADPH-d activity. It is also noted that VIP-LI and NADPH-d activity are colocalized In some nerve fibers (original magnification x600).
Discussion
atic nerve
In this study, we showed that the presence of NADPH-d activity in neurons and vascular endothelium was a finding common to the rat, guinea pig, dog, and human colocalized
pancreas and that NADPH-d activity was with VIP-L1 within a part of intrapancre-
Table 2. Percentage of Nerve Cell Bodies With NADPH-d Activity and/or VIP-LI in the Pancreas Nerve cell type NADF’H-d+, NADPH-d-, NADF’H-d+, NADPH-d-,
VIP+ VIP+ VIPVIP-
Rat
Guinea pig
Dog
Human
86 + 2 a&i 61+1 0.2 i 0.2
78 t 4 a&2 a*3 3-+1
16 + 6 66 f 5 lOk3 a+ i
53 t 2 23? 1 19?2 3fl
NOTE. The numbers shown for each type of neuron are percentages (mean + SE) of the total nerve cell bodies examined. +, positive; -, negatrve.
fibers and nerve
cell bodies.
Recent
studies
have presented strong evidence that NADPH-d corresponds to neuronal NOS. 3,4 Our present histochemical results, together with the evidence, suggest that the nerves and vascular endothelium of the pancreas may produce NO, which may work as a neuronal mediator and an endothelium-derived relaxing factor in the mammalian pancreas. The presence of several isoforms of NOS has been clarified.22-24 By biochemical characteristics, these isoforms have been classified into two major categories. One is designated as the constitutive NOS, present in neurons and vascular endothelium, and the other as the inducible NOS, present in macrophages, neutrophils, pancreatic islet cells, or hepatocytes.23-25 Recent reports suggest that the constitutive NOS is localized in the rat islet cells or in the cultured rat insulinoma cells and that NO produced in islet cells may be the
1006
SHIMOSEGAWA
mediator
of arginine-stimulated
Careful tion
observations
activity
of guanylate of cyclic
cyclase
guanosine
and the resultant
the only known
numerous
activity
in the rat islets,
obtained
of other
cells agrees with but
NADPH-d
activity
previous
disagrees
cells.25*26 There
animal
activity
in
ancy, but the possibility
pancreatic
should
endocrine
as a neuronal
activity parenchyma,
activity
ganglion
cells,
re-
cells by the activation
of
and it has been
suggested
pancreatic
acinar
are increased
cells,
intracellular
by acetylcholine,
levels
providing in acinar
cells. 36-38 However,
ported
that elevation
(at least
troprusside
release.39 As shown and nerve in the
It is, therefore,
have
nerve from been
with
NADPH-d
vascular
by nitrosourea
on Ca2+ fluxes
the neurotransmitter
could be roughly
grouped
walls of the mouse.28
they suggested a general capable of producing NO
the intracellular
signal
into the enteric
and parasym-
pathetic postganglionic nerves. Our findings indicate that intrinsic neurons of the mammalian pancreas should also be added to the nerve systems that may produce NO. Nerve bundles
in intralobular
and interlobular
nective tissues of all animal species examined tained numerous nonvaricose nerve fibers NADPH-d activity, suggesting that extrapancreatic
con-
neurons
rat and guinea were
coexpressed
pig pancreas, coexpressed
or neuromo-
transduction
by NO and the biological pancreas.
and VIP-LI, suggesting that these duce both NO and VIP as neuronal VIP-L1
nerve fibers not only in
it is important action
pancreatic
is localized in nerve cell bodies pharynx, bladder walls, pelvic
or ni-
or amylase
study, were distributed
role of NO in the pancreas,
induced exocrine
re-
but also in ducts and acini in the pan-
creas. To establish clarify
it has been
in the p resent
activity
systems
dulator
of cGMP
has no effect
NADPH-d activity within the tongue,
and the intestinal
bom-
cyclase
The present study of colocalization and nerve cell bodies confirmed that
Based on these observations, rule that peripheral neurons
of cGMP
cholecystokinin,
regarded as the parasympathetic postganglionic. Recently, it has been shown by Grozdanovic et al. that
nerve plexuses,
that gua-
nylate cyclase-dependent mechanisms are involved in the insulin secretion from islet B cells.35 In dispersed
phore,
were diffusely
which
path-
that NO
endocrine
conceivable that at least a part of intrapancreatic fibers stained for NADPH-d may have originated the intrapancreatic
muscle
confirmed
and A231 87, a calcium ionoproof of the presence of guanylate
were shown
examined.
cyclase
signal transduction
are
physalaemin,
mediator.
in the pancreatic
guanylate
smooth
produc-
(cGMP)
besin,
the pancreatic
fibers with NADPH-d
of all the animals
on rat
laxes arterial
intracellular
No. 4
showing
be considered
that NO regulates
cell bodies with NADPH-d
Our
for this discrep-
in the rat pancreas) functions
species.
in pancreatic
others
is no clear explanation
ob-
was not
observations
with rat
termi-
were
this finding
of no NADPH-d
pancreas2’
nerve
for NADPH-d
although
in the pancreas
observation
dotlike
Vol. 105,
monophosphate
way for NO. 30-34 It has been
a strong
pancreas
tion
species
with
Nerve
vation
but no
nals
within
the localiza-
islet cells,
By contrast,
distributed
secretion.25’26
was seen in the islet cells of any animal
examined. served
insulin
were made to clarify
of NADPH-d
staining
acinar
GASTROENTEROLOGY
ET AL.
to
pathway
of NO on the in nerve fibers a part of intra-
NADPH-d
activity
neurons may promediators. In the
NADPH-d in a large
activity
and
proportion
of
nerve cell bodies within the ganglia (about 80%). However, in the dog and human pancreas, only about 16% and 53% of ganglion cell bodies, respectively, coexpressed them, although in both animal species more than 75% of nerve cell bodies showed VIP-LI. These observations strongly suggest that VIP-containing rons in the mammalian pancreas could be divided
neuinto
conwith ori-
two groups: neurons capable of synthesizing both VIP and NO and neurons synthesizing only VIP. Most
gins with the enzyme activity may also contribute to the innervation of the pancreas. In rats, NADPH-d activity has been shown in the nerve cell bodies of the sensory ganglia,‘” but not in the nerve cell bodies of the sympathetic ganglia. ‘* It is possible, therefore, that nerve fibers with sensory origins may constitute a part of the NO-synthesizing nerve system in the mammalian pancreas. Species differences were evident in the distribution of NADPH-d-positive nerve fibers in the pancreas, suggesting that NO may exert different modes of action on the pancreas from species to species. The acti-
nerve cell bodies in the rat and guinea pig pancreas correspond with the first type, whereas in the dogpancress, the latter type neurons are dominant. Because the variation of the ratio of the two types of VIP neurons was relatively small in the respective animal species, the ratio may be genetically determined from species to species. The importance of VIP in the mammalian pancreas was suggested by the presence of VIP-L1 in most neurons in the pancreas, irrespective of animal species. Meanwhile, the existence of NADPH-d activity in only a part of VIP-L1 neurons in the dog pancreas suggests that NO may exert a supple-
October 1993
ment-ary
NADPH-D ACTIVITY IN THE PANCREAS
role for VIP or may bear some specialized
in the pancreas of at least the dog species. By immunohistochemistry, it has been that
NADPH-d
choline
is colocalized
acetyltransferase
in certain
in the brain.40T4’ Recently, LI and VIP-L1
has been
teric neurons,15
mdicating
sion and coproduction to th.e intrinsic but instead
systems
needed
to
meaning
neurons
clarify
suggested
neuropeptide groups
of neurons
the colocalization shown
Y or
of NOS-
in the guinea
that the possible
pig encoexpres-
of NO and VIP are not specific
represent
nervous
with
role
of the mammalian a general
of digestive
pancreas,
rule for the intrinsic
organs.
the
physiological
of the possible
coproduction
Further
study
and
biological
is
fiber types innervating the taenia of the guinea-pig caecum. Cell Tissue Res 1992;270: 125- 137. 16. ShimosegawaT, Moriizumi S, Koizumi M, Kashimura J, Yanaihara N, Toyota T. lmmunohistochemical demonstration of galaninlike immunoreactive nerves in the human pancreas. Gastroenterology 1992; 102~263-27 1. 17. Larsson LI. Innervation of the pancreas by substance P. enkephalin. vasoactive intestinal polypeptide and gastrin/CCK immunoreactive nerves. J Histochem Cytochem 1979;27: 1283- 1284. 18. Bishop AE, Polak JM, Green IC, Bryant MG, Bloom SR. The location of VIP in the pancreas of man and rat. Diabetologia 1980; 18:73-78. 19. DeGiorgio R, Sternini C, Anderson K, Brecha N, Go VLW. Tissue distribution and innervation pattern of peptide immunoreactivities in the rat pancreas. Peptides 1992;13:91-98. 20.
of NO and VIP.
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Received January 13, 1993. Accepted June 3, 1993. Address requests for reprints to: Tooru Shimosegawa, M.D., Third Department of Internal Medicine, Tohoku University School of Medicine, l-l Seiryo-machi, Aoba-ku, Sendai, Miyagi 980, Japan. The autopsy specimens of the human pancreas used in this study were supplied by the Department of Pathology and the surgical specimens by the First Department of Surgery, Tohoku University School of Medicine, Sendai, Japan.