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Hormonal stimulation of cAMP-dependent protein kinase in rat pancreas
Vol.
95,
No.
2, 1980
July
31,
1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
553-561
Pages
HORMONAL STIMULATION 0. Holian,
OF CAMP-DEPENDENT PROTEIN KINASE IN RAT PANCREAS
Ph.D.,
C. T. Bombeck,
M.D.,
Lloyd
M. Nyhus,
M. D.
From the Department of Surgery, University of Illinois at the Medical Center, The Abraham Lincoln School of Medicine, Chicago, Illinois
Received
June 6,198O SUMMARY
Rat pancreas possesses a CAMP-dependent protein kinase enzyme which is inhibited by the protein kinase inhibitor from bovine heart. Incubation of rat pancreas tissue in the presence of secretin and CCK-PZ resulted in an increase of intracellular CAMP and activation of the CAMP-dependent protein kinase. CCK-OP, a pure synthetic analog of CCK-PZ, did not stimulate cellular CAMP production or protein kinase activation. There was correlation between the ability of a given dose of hormone to stimulate CAMP formation and activate the protein kinase enzyme. It is believed that the stimulatory effect of CCK-PZ is due to secretin contamination of this hormonal preparation. Many of theeffects tissues
are
dent
protein
with
the
of cyclic
believed
to be mediated
kinase
(1).
regulatory The catalytic
resulting
in an intracellular (3)
can be studied
in vitro
exocrine
CAMP levels agents
pancreas.
in tissue
CCK has been guinea
using
cells
pig
levels
protein
the
activation
slices.
as the
second
and vasoactive
isolated
from
guinea
(CCK) had no effect of cyclic
kinase
(2).
of protein
Soderling
kinase
of hormonally
intestinal pigs
in the
by CAMP
stimu-
peptide
(4,5).
monophosphate
cyclase
catalytic
substrate,
increased
Cholinergic
on CAMP levels,
guanosine
adenylyl
by combining
an active
action
messenger
mammalian
of CAMP-depen-
appropriate
of hormonal
tissue
shown to stimulate
but caused (cGMP).
pancreas
an
However
of rat
and
(6,8).
The aim of the present dent
protein
enzyme and liberating
hormonal
Secretin
(cAMP)in
in the activity
phosphorylates
that
and cholecystokinin
increase
of the
implicated
in acinar
by changes
expression
showed
monophosphate
AMP activates
subunit
and associates
lated
Cyclic
subunit
subunit.
CAMP has been
adenosine
kinase
work
by stimulation
was to study
the activation
of endogenous
CAMP formation
of CAMP-depenin the
presence
0006-291X/80/140553-09$01.00/0
553
Copyright Q 1980 b-v Academic Press, Inc. All rrghts of reproduction in an-v form reserved.
Vol.
95, No.
2, 1980
of hormones. with
BIOCHEMICAL
It was of special
interest
cholecystokinin-pancreozymin
cholecystokinin
AND
BIOPHYSICAL
RESEARCH
to compare
the effects
(CCK-PZ),
and a synthetic
COMMUNICATIONS
of secretin
octapeptide
of
(CCK-OP). MATERIALS AND METHODS
Tissue Incubation. Pancreata were obtained from male Sprague-Dawley rats weighing 150 to 200 gm fed on a standard meal ad libitum. Prior to the experiThe rats were killed by a blow to the ment, the rats were fasted for 48 hours. head; the pancreas quickly removed, dissected free from fat and mesentery and used immediately. The pancreas was cut into small pieces and placed in Ringer's bicarbonate buffer, pH 7.4, containing 1 mg/ml glucose and 0.5 mM 3-isobutylThe tissue was preincubated at 37O C for ten minutes l-methyl xanthine (IMX). with mild shaking. At the end of the preincubation period, the tissue was transferred to fresh buffer containing the appropriate hormones and incubated for additional ten minutes at 37O C. Two to three pieces of tissue, approximately in 5 ml of buffer. At the end of the incubation 2 to 4 mm2, were incubated period, the tissue was quickly removed, frozen in liquid nitrogen, and subsequently stored under liquid nitrogen. Enzyme Preparation. Frozen tissue was pulverized in liquid nitrogen and the pulverized powder homogenized in ten volumes of 10 mM potassium phosphate buffer, pH 6.5, containing 10 mM ethylene diamine tetraacetate (EDTA) and l165cmM IMX. The homogenate was centrifuged at 27,000 x g for 20 minutes at The supernatant fraction was used as the enzyme preparation. Protein kinase assay was performed imnediately after enzyme preparation. Protein Kinase Assay. The reaction was started by adding 5 to 20 ~1 of the enzyme preparation to 50 ~1 of a solution containing 17 mM potassium phosphate buffer,3$ H 6.8, 10 mg/ml histone (Sigma type II-A), 6 mM magnesium acetate, 0.33 mM ATP-y p (20 to 50 counts per minute/pmole) in the presence and in the absence of 2 PM CAMP. The reaction mixture was incubated at 30o C for 5 minutes and the reaction terminated by addition of 1 ml of ice cold 10% trichloroacetic acid (TCA). The formed precipitate was collected by filtration on Whatman GFlC glass fiber filters, washed four times with 2 ml portions of ice cold 10% TCA, and counted in 5 ml of Bray's solution (9) in a Packard Tri-Carb liquid scintillation counter. The protein kinase activity was expressed as pmoles of 32p incorporated into histone per milligram of protein per minute. The protein kinase activity ratio was expressed as the ratio of protein kinase activity in the absence of added CAMP to protein kinase tivity in the presence of 2 PM CAMP. In each assay nons ecific binding of 35 p to histone was determined by measuring the amount of 3! P bound to denatured enzyme. The value obtained was used as zero time incubation, and was subtracted from all other values. CAMP Assay. Frozen tissue, previously incubated with and without hormones, was homogenized in 3 ml of ice cold 6% TCA and 6000 dpm of 3H-cAMP were added to determine recovery. The homogenate was centrifuged at 10,000 x g for 30 minutes at 4O C. The supernatant fraction was applied to a Dowex 50-H+ form column, 100 to 200 mesh, 0.9 x 15 cm, which had been equilibrated with O.lN HCl. The column was eluted with O.lN HCl, the CAMP elution profile determined, and the fraction containing CAMP was collected and lyophilized to dryness. The lyophilized fraction was resuspended in 1 ml of water and the concentration of CAMP was determined against a standard curve by the method of Gilman (10). The CAMP values obtained were corrected for recovery and expressed as pmoles of CAMP per milligram of protein. Protein Determination. of Lowry (11).
Protein
concentration
554
was determined
by the method
Vol.
95, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Materials. Type II-A histone, CAMP-dependent protein kinase inhibitor from bovine heart, CAMP, ATP, IMX, and binding protein were purchased from porcine preparation of secretin and the Sigma Chemical Co. The natural CCK-PZ were purchased from the Karolinska Institute, Stockholm, Sweden; this supplier states that each ampule containing 75 U of CCK-PZ also contains 0.7 U of secretin. CCK-OP wgs a gift of the Squibb Institute for Medical Research; ATP-~32P and CAMP- H were purchased from the New England Nuclear Corporation. All other chemicals used were of the highest purity commercially available. RESULTS Control caused
Studies.
of exogenous
a concentration-dependent
histone
(Fig.
1).
increase
Activation
CAMP concentration tion
Addition
in pmoles
of protein
of 0.05
CAMP to the
kinase
PM and was optimal
reaction
mixture
of 32P incorporated
was already
into
apparent
at 0.4 MM, when the
at a concentra-
of the enzyme was 200 ug protein. The effects
kinase
activity
reaction
are
shown
was carried
centration It
of protein
between
out
probably holoenzyme.
effect caused
in Fig. for
five
(12,13)
In all
minutes
that
on the protein by stabilization
Increasing
and time
2.
100 to 500 vg per
has been shown
stabilizing
concentration
subsequent
at 30'
on protein
experiments
C maintaining
the
protein
con-
tube. in some tissues
kinase
activity
of dissociation
concentrations
addition ratio. of the
of NaCl present
CAMP
Effect of was incubated cAMP concentrations, point was determined of two others.
of incubation
This protein during
effect
is
kinase tissue
(PM)
CAMP on protein kinase activity. for 5 minutes at 30° C in the and protein kinase activity was in triplicate, and this experiment
555
of NaCl has a
The enzyme (200 vg presence of varying determined. Each is representative
homo-
Vol.
95,
No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
60.
I -0
50 MINUTES
100
OF INCUBATION
pq
I 200
I 800
400
PROTEIN
Effects of incubation time and protein concentration on the F$S%Ginase activity In the top curve 100 ug protein were incubated for different times at iO" C in the presence and absence of 2 UM CAMP. In the bottom curve varying amounts of protein were incubated for 5 minutes at 300 C in the presence and absence of 2 LIM CAMP. Each point was determined in triplicate and each experiment is representative of two others. The dashed line represents values in the absence of CAMP; solid line represents values in the presence of 2 LIM CAMP.
genization
caused
indicating
an
to
dissociation
in
the
by
of
the
activity
component
kinase
portion
protein,
Effects.
As
with
a secretin
of
ratio
of
holoenzyme.
the
the
NaCl
protein
kinase
inhibitor
protein
kinase
shown
secretin
was
no
further
to
1o-4
M.
in
tissue
of
CAMP
of were
increase The
CAMP a response
in
natural level
(Fig.3),
enzyme was
kinase from
probably
due
therefore
activity
bovine
activity
of
the
Fig.
5,
omitted
was
heart
inhibited
(Fig.
approached
cAMP
higher same
CAMP
CCK-PZ.
10m7
M.
The
level
4).
that
nine
times
when
in
concentrations of
magnitude
556
was
the
At the
tissue
rose
already
apparent
basal
was level.
concentration
CCK-PZ of
the
concentration
secretin of
in
increase
secretin
preparation
order
levels
When
approximately
porcine but
in or
concentration
levels
produce
catalytic
protein
protein
incubation
tissue
kinase
CAMP.
Hormonal after
protein
experiments.
inhibitor of
in the
cAMP-stimulated
of
absence
at
in
a CAMP-dependent
80 pg
increase
increase
following The
an
also
CCK-PZ as
caused were
obtained
There was
raised
an
increase
required with
low5
to secretin.
M,
Vol.
95, No.
03
BIOCHEMICAL
2, 1980
B
05
’
NaCl
Figure 3. centrations The enzyme 5 minutes experiment
20
IO
AND
zr; 04
’
30
BIOPHYSICAL
40
(M)
RESEARCH
PROTEIN
KINASE
COMMUNICATIONS
INHIBITOR
(pig
protein)
Effect of NaCl on protein kinase activity ratio. Varying conof NaCl were present during homogenization of the tissue. was incubated in the presence and absence of 2 nM CAMP for Each point was determined in triplicate, and this at 30° C. is representative of two others.
Figure 4. Effect of bovine heart protein kinase inhibitor on protein kinase activity. The enzyme (47 ug protein) was incubated with varying concentrations of the protein kinase inhibitor in the presence of 2 nM CAMP for 5 minutes at 30° C. The protein kinase activity in the absence of 2 uM CAMP was the same as that in the presence of 75 ng protein of the Protein kinase activity is expressed as per protein kinase inhibitor. cent of the activity obtained with 2 nM CAMP in the absence of protein kinase inhibitor. The
synthetic
carboxy-terminal
cant
changes
were
the
same
octapeptide
CAMP tissue
in as
levels.
At
(CCK-OP) 10 -4
did
M CCK-OP,tissue
not
produce CAMP
signifilevels
controls. ‘30 80
r-
SECRETIN
HORMONE
CONCENTRATION(M)
Figure 5. Effect of hormone concentration on CAMP levels. The tissue was prelncubated with buffer alone for 10 minutes and then incubated with hormones for additional 10 minutes. Each point is a mean t s.e. of three separate experiments, and each experimental value was obtained from quadruplicate tissue samples.
557
Vol.
95. No.
2, 1980
BIOCHEMICAL
I
Table.
EFFECT
OF HORMONES Protein
Hormone Concentration
AND
(M)
BIOPHYSICAL
ON PROTEIN
Kinase
RESEARCH
ACTIVITY RATIO
KINASE
Activity
COMMUNICATIONS
Ratio
(-cAMP/+cAMP)
Secretin
CCK-PZ
CCK-OP
0.188 -t .006
0.188 + .006
0.245 f .017
1O-8 -7 10
0.220
0.198 f .033
0.274 + .019
0.271 T .OOO
0.233 t .012
0.252 + .009
lo-6
0.315 k .016
0.245 f .022
0.288 T .029
10-5
0.419 ?- .OlO
0.300 t .036
0.293 t .025
lo-4
0.482 ?r .OOO
0.355 + .036
0.273 i .029
0
*
.OlO
Tissue was preincubated with buffer alone for 10 minutes, and then incubated with hormones for additional 10 minutes. Protein kinase Each activity ratio was determined as described under methods. point is a mean + s.e. of three separate experiments, and each experimental value was obtained from quadruplicate tissue samples.
Incubation
of pancreatic
concentration-dependent The ratio
increase
increased
.OOO in the
from
presence
CCK-PZ produced
The synthetic
kinase
activity
of 10
caused
by animal
with
in the + 0.066
-4
secretin protein
when tested
kinase
produce
between
in the CCK-OP experiments and experimental
CCK-PZ produced activity
any added
Incubation
in the protein not
or kinase
without
M secretin.
CCK-OP did
ratio
ratio
0.188
an increase
.036.
activity
tissue
ratio
hormone
of tissue activity
with
ratio
I).
+
10m4 M
to 0.355
change
10m8 to 10s4 M.
The higher
be explained
(Table
to 0.482
any significant
cannot
a
+
in protein basal
but may have been
variations. DISCUSSION
Stimulation changes fluid
of exocrine
in tissue
levels
and bicarbonate
system
(E-20).
of CAMP during stimulation
pancreatic
of CAMP (14). secretion
On the other CCK-stimulated of adenylyl
administration
of the
of increased
CAMP levels
secretion
are
is
mediated
hand,
although
has been shown that through data
enzyme secretion
cyclase hormone
It
activity
the point
(4),some
and increased
(8,21-24). believed
is thought
The metabolic to be expressed
558
to be related
to
stimulation
of
CAMP-adenylyl
cyclase
to the noninvolvement reports cellular
have shown CAMP after
and functional through
the
effects
activation
Vol.
95, No.
2, 1980
BIOCHEMICAL
of CAMP-dependent kinase
protein
cells
confirmed
that
isolated the
tains
a protein
study
demonstrates
using
an in vitro
enzyme which
hormonal
There hormones
in elevating
enzyme.
When it
between tissue
intracellular
CAMP.
subsequent
stimulation
assumed
enzyme This
of fluid
is
responsible for
known
that
secretin. the
of secretin
weights
of the
CCK-PZ preparation
This
con-
protein
kinase
secretin
buffer levels
with
secret
of CAMP.
as was CCK-PZ.
the degree
stimulation
In
analog
only
by stimulation the
of
formed
of CAMP and protein
contains
can account
for
CCK-PZ preparation.
559
that enzyme
kinase
production
degree
two different the
hormonal
secretion
is
activation,
It is
Taking
into
that
and each
2 x 10e3 doles of stimulation
of
with
(see Materials)
can be calculated
approximately the
the
of
activates
kinase
by secretin.
in the CCK-PZ preparation it
secretin
of enzyme secretion.
contaminated
two hormones,
with
indicate
of pancreatic
stimulants
that
a protein
The results
protein
production
in increased
CAMP activates
equipotent
kinase
CAMP-dependent
concept
resulting
stimulation
of the
the protein
of endogenous
current
pancreas,
is
of potency
of the
(CCK-PZ and CCK-OP)
CCK-PZ preparation
amount
the
the stimulation
CCK-PZ and CCK-OP are
mMole of the
pancreas
has
In additian;this
in tissue
and activating
secretion.
for
since
the molecular
and
Our study
of rat
a stimulant
between levels
that
newly
moiety
the
(25-27)
CAMP levels.
in the
of cholecystokinin
account
rats
(28).
bicarbonate
increase
strengthen
preparations
the
pigs
by CAMP.
in Ringer's
relationship
findings
cyclase
responsible
from
protein
-4 M CCK-OP, the synthetic to 10
CAMP tissue
is
CAMP, the present
not
of guinea
as potent
low8
can be achieved
which
of pancreata
of the CAMP-dependent
tissue
loo-fold
was a general
an adenylyl
of a CAMP-dependent
stimulated
a dose-dependent
not elevate
activity
is
COMMUNICATIONS
system.
ranges
did
RESEARCH
of the homogenate
stimulation
was approximately
CCK-PZ,
kinase
fraction
of pancreatic
concentration
The presence
the pancreata
supernatant
or CCK-PZ produced
Secretin
BIOPHYSICAL
in homogenates from
kinase
Incubation tin
kinases.
has been demonstrated
in acinar
AND
found
of with
Vol.
95, No.
2. 1980
Complete is
possible
activation that
of the protein resulting
reassociation
activity
activity
ratio findings
pancreatic
cholecystokinin
both confirm
kinase
during
RESEARCH
COMMUNICATIONS
catalytic
tissue
and regulatory
homogenization
subunits
and assay,
Preliminary
experiments
indicate
tissue
homogenization
results
in a higher
that
enzyme secretion,
CAMP is
and presence
of hormones.
not
during
involved
and stimulation to secretin
It
enzyme was not achieved.
ratio.
in the absence
may be attributed
BIOPHYSICAL
of the
enzyme occurs
of 0.5 M NaCl during
the present lated
kinase
AND
of the protein
a rapid
in a lower
presence kinase
BIOCHEMICAL
of adenylyl
contamination
that protein In summary,
hormonally cyclase of this
stimuby
hormonal
preparation. ACKNOWLEDGEMENT We wish to thank Mrs. Cathy Ruiz for her expert technical This work was supported in part by PHS-AM 20838-01 grant from Institutes of Health.
assistance. the National
REFERENCES
:: i: 5. 6. 7. 8. 9. :::
Kuo,J.F., Greengard, P. (1969) Proc. Natl. Acad. Sci. USA 64, 1349. Krebs, E.G. (1972) Curr. Top. Cell Regul. 5, 99-133. Soderling, T.R., Corbin, J.D., Park, C.R. 71973) J. Biol. Chem. =,1822-1829 Gardner, J.D., Conlon, T.P., Adams, T.D. (1976) Gastroenterology 7&29-35. Gardner, J.D., Conlon, T.P., Fink, M.L., et al. (1976) Gastroenterology 71,965-970. J. (1972) Rev. Can. Biol. x,253-257. Mass, C., Morisset, J., Dunnigan, Bonting, S.L. (1972) Biochim, et Biophys. Rutten,W.J..DePont, J.J.H.H.M., Acta z,201-213. Gardner, J.D. (1975) in Gastrointestinal Klaeveman, H.L., Conlon, T.P., Ed.) p 321-344, University of Texas Press, Austin, Hormones (Thompson,J.C., and London B$*'G A (1960)'Anal Biochem 1 279 Gilmin,'A:G. (1970) P&c. Natl.'AFid, Sci. 67, 305-312. Lowry, O.H., Rosebrough, N.J., Farr, A.L., et al. (1951) J. Biol. Chem.
m,265-275. 12. Corbin, J.D., 13. 14. :;: 17. 18. 19. 20.
Park, C.R. (1973) J. Biol. Chem. 248, Soderling, T.R., 1813-1821. Keely, S.L.,Soderling, T.R., et al. (1975) in Advances in Corbin, J.D., Cyclic Nucleotide Research (Drummond,G.I., Greengard, P., Robison, ,G.A. Eds.) Vol. 5, p 265-279 Raven Press, New York. Kimberg, D.V. (1974) Gastroenterology 67, 1023-1064. Tompkins, R.K., Kuchenbecker, S.L. (1973) J. Surg. Res. x,172-176. G. (1974) Life Sci. I& 631-639. Heisler, S., Grondin, G., Forget, Deschodt-Lanckman, M., Robberecht, P., DeNeef, P., et al. (1975) Gastroenterology 68, 318-325. Lemon, M.J.C., Bhoola, K.D. (1975) Biochim. et Biophys. Acta 385,101-113. Domschke, S., Konturek, S.J.,Domschke, W., et al. (1975) Proc. Sot. Exp. Biol. Med. 150, 773-779. Domschke, S., Domschke, W.,Konturek, S., et al. (1976) Gastroenterology
z,533-536.
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Vol.
95, No.
2, 1980
BIOCHEMICAL
AND
BlOPHYSlCAL
RESEARCH
21. Case,R.M.,Johnson, M., Scratchert, T., et al. (1972) J. 669-684. 22. Marois, C., Morisset, J., Dunnigan, J. (1972) Rev. Can. 23. Rutten, W.J., DePont, J.J.H.H.M., Bonting, S.L. (1972) Acta =,201-213. 24. Kempen, H.J.M., DePont, J.J.H.H.M., Bonting, S.L. (1974) Biophys. Acta 370, 573-584 25. VanLeemput-Coutrez, M., Camus, J., Christophe, J. (1973) Res. Commun. 54, 182-190. G. (1957) 26. Cenatiempo, Y., Margeat, P., Marchis-Mauren, 865-873. J. (1975) Biochem. 27. Lambert, M., Camus, J., Christophe, 1755-1758. 28. Jensen, R.T.,Gardner, J.D. (1978) Gastroenterology 75,
561
COMMUNICATIONS
Physiol.
223,
Biol. ~,253-257. Biochim. et Biophys. Biochim.
et
Biochem.
Biophys.
Biochimie,
57,
Pharmacol.
24,
806-817.
95,
No.
2, 1980
July
31,
1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
553-561
Pages
HORMONAL STIMULATION 0. Holian,
OF CAMP-DEPENDENT PROTEIN KINASE IN RAT PANCREAS
Ph.D.,
C. T. Bombeck,
M.D.,
Lloyd
M. Nyhus,
M. D.
From the Department of Surgery, University of Illinois at the Medical Center, The Abraham Lincoln School of Medicine, Chicago, Illinois
Received
June 6,198O SUMMARY
Rat pancreas possesses a CAMP-dependent protein kinase enzyme which is inhibited by the protein kinase inhibitor from bovine heart. Incubation of rat pancreas tissue in the presence of secretin and CCK-PZ resulted in an increase of intracellular CAMP and activation of the CAMP-dependent protein kinase. CCK-OP, a pure synthetic analog of CCK-PZ, did not stimulate cellular CAMP production or protein kinase activation. There was correlation between the ability of a given dose of hormone to stimulate CAMP formation and activate the protein kinase enzyme. It is believed that the stimulatory effect of CCK-PZ is due to secretin contamination of this hormonal preparation. Many of theeffects tissues
are
dent
protein
with
the
of cyclic
believed
to be mediated
kinase
(1).
regulatory The catalytic
resulting
in an intracellular (3)
can be studied
in vitro
exocrine
CAMP levels agents
pancreas.
in tissue
CCK has been guinea
using
cells
pig
levels
protein
the
activation
slices.
as the
second
and vasoactive
isolated
from
guinea
(CCK) had no effect of cyclic
kinase
(2).
of protein
Soderling
kinase
of hormonally
intestinal pigs
in the
by CAMP
stimu-
peptide
(4,5).
monophosphate
cyclase
catalytic
substrate,
increased
Cholinergic
on CAMP levels,
guanosine
adenylyl
by combining
an active
action
messenger
mammalian
of CAMP-depen-
appropriate
of hormonal
tissue
shown to stimulate
but caused (cGMP).
pancreas
an
However
of rat
and
(6,8).
The aim of the present dent
protein
enzyme and liberating
hormonal
Secretin
(cAMP)in
in the activity
phosphorylates
that
and cholecystokinin
increase
of the
implicated
in acinar
by changes
expression
showed
monophosphate
AMP activates
subunit
and associates
lated
Cyclic
subunit
subunit.
CAMP has been
adenosine
kinase
work
by stimulation
was to study
the activation
of endogenous
CAMP formation
of CAMP-depenin the
presence
0006-291X/80/140553-09$01.00/0
553
Copyright Q 1980 b-v Academic Press, Inc. All rrghts of reproduction in an-v form reserved.
Vol.
95, No.
2, 1980
of hormones. with
BIOCHEMICAL
It was of special
interest
cholecystokinin-pancreozymin
cholecystokinin
AND
BIOPHYSICAL
RESEARCH
to compare
the effects
(CCK-PZ),
and a synthetic
COMMUNICATIONS
of secretin
octapeptide
of
(CCK-OP). MATERIALS AND METHODS
Tissue Incubation. Pancreata were obtained from male Sprague-Dawley rats weighing 150 to 200 gm fed on a standard meal ad libitum. Prior to the experiThe rats were killed by a blow to the ment, the rats were fasted for 48 hours. head; the pancreas quickly removed, dissected free from fat and mesentery and used immediately. The pancreas was cut into small pieces and placed in Ringer's bicarbonate buffer, pH 7.4, containing 1 mg/ml glucose and 0.5 mM 3-isobutylThe tissue was preincubated at 37O C for ten minutes l-methyl xanthine (IMX). with mild shaking. At the end of the preincubation period, the tissue was transferred to fresh buffer containing the appropriate hormones and incubated for additional ten minutes at 37O C. Two to three pieces of tissue, approximately in 5 ml of buffer. At the end of the incubation 2 to 4 mm2, were incubated period, the tissue was quickly removed, frozen in liquid nitrogen, and subsequently stored under liquid nitrogen. Enzyme Preparation. Frozen tissue was pulverized in liquid nitrogen and the pulverized powder homogenized in ten volumes of 10 mM potassium phosphate buffer, pH 6.5, containing 10 mM ethylene diamine tetraacetate (EDTA) and l165cmM IMX. The homogenate was centrifuged at 27,000 x g for 20 minutes at The supernatant fraction was used as the enzyme preparation. Protein kinase assay was performed imnediately after enzyme preparation. Protein Kinase Assay. The reaction was started by adding 5 to 20 ~1 of the enzyme preparation to 50 ~1 of a solution containing 17 mM potassium phosphate buffer,3$ H 6.8, 10 mg/ml histone (Sigma type II-A), 6 mM magnesium acetate, 0.33 mM ATP-y p (20 to 50 counts per minute/pmole) in the presence and in the absence of 2 PM CAMP. The reaction mixture was incubated at 30o C for 5 minutes and the reaction terminated by addition of 1 ml of ice cold 10% trichloroacetic acid (TCA). The formed precipitate was collected by filtration on Whatman GFlC glass fiber filters, washed four times with 2 ml portions of ice cold 10% TCA, and counted in 5 ml of Bray's solution (9) in a Packard Tri-Carb liquid scintillation counter. The protein kinase activity was expressed as pmoles of 32p incorporated into histone per milligram of protein per minute. The protein kinase activity ratio was expressed as the ratio of protein kinase activity in the absence of added CAMP to protein kinase tivity in the presence of 2 PM CAMP. In each assay nons ecific binding of 35 p to histone was determined by measuring the amount of 3! P bound to denatured enzyme. The value obtained was used as zero time incubation, and was subtracted from all other values. CAMP Assay. Frozen tissue, previously incubated with and without hormones, was homogenized in 3 ml of ice cold 6% TCA and 6000 dpm of 3H-cAMP were added to determine recovery. The homogenate was centrifuged at 10,000 x g for 30 minutes at 4O C. The supernatant fraction was applied to a Dowex 50-H+ form column, 100 to 200 mesh, 0.9 x 15 cm, which had been equilibrated with O.lN HCl. The column was eluted with O.lN HCl, the CAMP elution profile determined, and the fraction containing CAMP was collected and lyophilized to dryness. The lyophilized fraction was resuspended in 1 ml of water and the concentration of CAMP was determined against a standard curve by the method of Gilman (10). The CAMP values obtained were corrected for recovery and expressed as pmoles of CAMP per milligram of protein. Protein Determination. of Lowry (11).
Protein
concentration
554
was determined
by the method
Vol.
95, No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
Materials. Type II-A histone, CAMP-dependent protein kinase inhibitor from bovine heart, CAMP, ATP, IMX, and binding protein were purchased from porcine preparation of secretin and the Sigma Chemical Co. The natural CCK-PZ were purchased from the Karolinska Institute, Stockholm, Sweden; this supplier states that each ampule containing 75 U of CCK-PZ also contains 0.7 U of secretin. CCK-OP wgs a gift of the Squibb Institute for Medical Research; ATP-~32P and CAMP- H were purchased from the New England Nuclear Corporation. All other chemicals used were of the highest purity commercially available. RESULTS Control caused
Studies.
of exogenous
a concentration-dependent
histone
(Fig.
1).
increase
Activation
CAMP concentration tion
Addition
in pmoles
of protein
of 0.05
CAMP to the
kinase
PM and was optimal
reaction
mixture
of 32P incorporated
was already
into
apparent
at 0.4 MM, when the
at a concentra-
of the enzyme was 200 ug protein. The effects
kinase
activity
reaction
are
shown
was carried
centration It
of protein
between
out
probably holoenzyme.
effect caused
in Fig. for
five
(12,13)
In all
minutes
that
on the protein by stabilization
Increasing
and time
2.
100 to 500 vg per
has been shown
stabilizing
concentration
subsequent
at 30'
on protein
experiments
C maintaining
the
protein
con-
tube. in some tissues
kinase
activity
of dissociation
concentrations
addition ratio. of the
of NaCl present
CAMP
Effect of was incubated cAMP concentrations, point was determined of two others.
of incubation
This protein during
effect
is
kinase tissue
(PM)
CAMP on protein kinase activity. for 5 minutes at 30° C in the and protein kinase activity was in triplicate, and this experiment
555
of NaCl has a
The enzyme (200 vg presence of varying determined. Each is representative
homo-
Vol.
95,
No.
2, 1980
BIOCHEMICAL
AND
BIOPHYSICAL
RESEARCH
COMMUNICATIONS
60.
I -0
50 MINUTES
100
OF INCUBATION
pq
I 200
I 800
400
PROTEIN
Effects of incubation time and protein concentration on the F$S%Ginase activity In the top curve 100 ug protein were incubated for different times at iO" C in the presence and absence of 2 UM CAMP. In the bottom curve varying amounts of protein were incubated for 5 minutes at 300 C in the presence and absence of 2 LIM CAMP. Each point was determined in triplicate and each experiment is representative of two others. The dashed line represents values in the absence of CAMP; solid line represents values in the presence of 2 LIM CAMP.
genization
caused
indicating
an
to
dissociation
in
the
by
of
the
activity
component
kinase
portion
protein,
Effects.
As
with
a secretin
of
ratio
of
holoenzyme.
the
the
NaCl
protein
kinase
inhibitor
protein
kinase
shown
secretin
was
no
further
to
1o-4
M.
in
tissue
of
CAMP
of were
increase The
CAMP a response
in
natural level
(Fig.3),
enzyme was
kinase from
probably
due
therefore
activity
bovine
activity
of
the
Fig.
5,
omitted
was
heart
inhibited
(Fig.
approached
cAMP
higher same
CAMP
CCK-PZ.
10m7
M.
The
level
4).
that
nine
times
when
in
concentrations of
magnitude
556
was
the
At the
tissue
rose
already
apparent
basal
was level.
concentration
CCK-PZ of
the
concentration
secretin of
in
increase
secretin
preparation
order
levels
When
approximately
porcine but
in or
concentration
levels
produce
catalytic
protein
protein
incubation
tissue
kinase
CAMP.
Hormonal after
protein
experiments.
inhibitor of
in the
cAMP-stimulated
of
absence
at
in
a CAMP-dependent
80 pg
increase
increase
following The
an
also
CCK-PZ as
caused were
obtained
There was
raised
an
increase
required with
low5
to secretin.
M,
Vol.
95, No.
03
BIOCHEMICAL
2, 1980
B
05
’
NaCl
Figure 3. centrations The enzyme 5 minutes experiment
20
IO
AND
zr; 04
’
30
BIOPHYSICAL
40
(M)
RESEARCH
PROTEIN
KINASE
COMMUNICATIONS
INHIBITOR
(pig
protein)
Effect of NaCl on protein kinase activity ratio. Varying conof NaCl were present during homogenization of the tissue. was incubated in the presence and absence of 2 nM CAMP for Each point was determined in triplicate, and this at 30° C. is representative of two others.
Figure 4. Effect of bovine heart protein kinase inhibitor on protein kinase activity. The enzyme (47 ug protein) was incubated with varying concentrations of the protein kinase inhibitor in the presence of 2 nM CAMP for 5 minutes at 30° C. The protein kinase activity in the absence of 2 uM CAMP was the same as that in the presence of 75 ng protein of the Protein kinase activity is expressed as per protein kinase inhibitor. cent of the activity obtained with 2 nM CAMP in the absence of protein kinase inhibitor. The
synthetic
carboxy-terminal
cant
changes
were
the
same
octapeptide
CAMP tissue
in as
levels.
At
(CCK-OP) 10 -4
did
M CCK-OP,tissue
not
produce CAMP
signifilevels
controls. ‘30 80
r-
SECRETIN
HORMONE
CONCENTRATION(M)
Figure 5. Effect of hormone concentration on CAMP levels. The tissue was prelncubated with buffer alone for 10 minutes and then incubated with hormones for additional 10 minutes. Each point is a mean t s.e. of three separate experiments, and each experimental value was obtained from quadruplicate tissue samples.
557
Vol.
95. No.
2, 1980
BIOCHEMICAL
I
Table.
EFFECT
OF HORMONES Protein
Hormone Concentration
AND
(M)
BIOPHYSICAL
ON PROTEIN
Kinase
RESEARCH
ACTIVITY RATIO
KINASE
Activity
COMMUNICATIONS
Ratio
(-cAMP/+cAMP)
Secretin
CCK-PZ
CCK-OP
0.188 -t .006
0.188 + .006
0.245 f .017
1O-8 -7 10
0.220
0.198 f .033
0.274 + .019
0.271 T .OOO
0.233 t .012
0.252 + .009
lo-6
0.315 k .016
0.245 f .022
0.288 T .029
10-5
0.419 ?- .OlO
0.300 t .036
0.293 t .025
lo-4
0.482 ?r .OOO
0.355 + .036
0.273 i .029
0
*
.OlO
Tissue was preincubated with buffer alone for 10 minutes, and then incubated with hormones for additional 10 minutes. Protein kinase Each activity ratio was determined as described under methods. point is a mean + s.e. of three separate experiments, and each experimental value was obtained from quadruplicate tissue samples.
Incubation
of pancreatic
concentration-dependent The ratio
increase
increased
.OOO in the
from
presence
CCK-PZ produced
The synthetic
kinase
activity
of 10
caused
by animal
with
in the + 0.066
-4
secretin protein
when tested
kinase
produce
between
in the CCK-OP experiments and experimental
CCK-PZ produced activity
any added
Incubation
in the protein not
or kinase
without
M secretin.
CCK-OP did
ratio
ratio
0.188
an increase
.036.
activity
tissue
ratio
hormone
of tissue activity
with
ratio
I).
+
10m4 M
to 0.355
change
10m8 to 10s4 M.
The higher
be explained
(Table
to 0.482
any significant
cannot
a
+
in protein basal
but may have been
variations. DISCUSSION
Stimulation changes fluid
of exocrine
in tissue
levels
and bicarbonate
system
(E-20).
of CAMP during stimulation
pancreatic
of CAMP (14). secretion
On the other CCK-stimulated of adenylyl
administration
of the
of increased
CAMP levels
secretion
are
is
mediated
hand,
although
has been shown that through data
enzyme secretion
cyclase hormone
It
activity
the point
(4),some
and increased
(8,21-24). believed
is thought
The metabolic to be expressed
558
to be related
to
stimulation
of
CAMP-adenylyl
cyclase
to the noninvolvement reports cellular
have shown CAMP after
and functional through
the
effects
activation
Vol.
95, No.
2, 1980
BIOCHEMICAL
of CAMP-dependent kinase
protein
cells
confirmed
that
isolated the
tains
a protein
study
demonstrates
using
an in vitro
enzyme which
hormonal
There hormones
in elevating
enzyme.
When it
between tissue
intracellular
CAMP.
subsequent
stimulation
assumed
enzyme This
of fluid
is
responsible for
known
that
secretin. the
of secretin
weights
of the
CCK-PZ preparation
This
con-
protein
kinase
secretin
buffer levels
with
secret
of CAMP.
as was CCK-PZ.
the degree
stimulation
In
analog
only
by stimulation the
of
formed
of CAMP and protein
contains
can account
for
CCK-PZ preparation.
559
that enzyme
kinase
production
degree
two different the
hormonal
secretion
is
activation,
It is
Taking
into
that
and each
2 x 10e3 doles of stimulation
of
with
(see Materials)
can be calculated
approximately the
the
of
activates
kinase
by secretin.
in the CCK-PZ preparation it
secretin
of enzyme secretion.
contaminated
two hormones,
with
indicate
of pancreatic
stimulants
that
a protein
The results
protein
production
in increased
CAMP activates
equipotent
kinase
CAMP-dependent
concept
resulting
stimulation
of the
the protein
of endogenous
current
pancreas,
is
of potency
of the
(CCK-PZ and CCK-OP)
CCK-PZ preparation
amount
the
the stimulation
CCK-PZ and CCK-OP are
mMole of the
pancreas
has
In additian;this
in tissue
and activating
secretion.
for
since
the molecular
and
Our study
of rat
a stimulant
between levels
that
newly
moiety
the
(25-27)
CAMP levels.
in the
of cholecystokinin
account
rats
(28).
bicarbonate
increase
strengthen
preparations
the
pigs
by CAMP.
in Ringer's
relationship
findings
cyclase
responsible
from
protein
-4 M CCK-OP, the synthetic to 10
CAMP tissue
is
CAMP, the present
not
of guinea
as potent
low8
can be achieved
which
of pancreata
of the CAMP-dependent
tissue
loo-fold
was a general
an adenylyl
of a CAMP-dependent
stimulated
a dose-dependent
not elevate
activity
is
COMMUNICATIONS
system.
ranges
did
RESEARCH
of the homogenate
stimulation
was approximately
CCK-PZ,
kinase
fraction
of pancreatic
concentration
The presence
the pancreata
supernatant
or CCK-PZ produced
Secretin
BIOPHYSICAL
in homogenates from
kinase
Incubation tin
kinases.
has been demonstrated
in acinar
AND
found
of with
Vol.
95, No.
2. 1980
Complete is
possible
activation that
of the protein resulting
reassociation
activity
activity
ratio findings
pancreatic
cholecystokinin
both confirm
kinase
during
RESEARCH
COMMUNICATIONS
catalytic
tissue
and regulatory
homogenization
subunits
and assay,
Preliminary
experiments
indicate
tissue
homogenization
results
in a higher
that
enzyme secretion,
CAMP is
and presence
of hormones.
not
during
involved
and stimulation to secretin
It
enzyme was not achieved.
ratio.
in the absence
may be attributed
BIOPHYSICAL
of the
enzyme occurs
of 0.5 M NaCl during
the present lated
kinase
AND
of the protein
a rapid
in a lower
presence kinase
BIOCHEMICAL
of adenylyl
contamination
that protein In summary,
hormonally cyclase of this
stimuby
hormonal
preparation. ACKNOWLEDGEMENT We wish to thank Mrs. Cathy Ruiz for her expert technical This work was supported in part by PHS-AM 20838-01 grant from Institutes of Health.
assistance. the National
REFERENCES
:: i: 5. 6. 7. 8. 9. :::
Kuo,J.F., Greengard, P. (1969) Proc. Natl. Acad. Sci. USA 64, 1349. Krebs, E.G. (1972) Curr. Top. Cell Regul. 5, 99-133. Soderling, T.R., Corbin, J.D., Park, C.R. 71973) J. Biol. Chem. =,1822-1829 Gardner, J.D., Conlon, T.P., Adams, T.D. (1976) Gastroenterology 7&29-35. Gardner, J.D., Conlon, T.P., Fink, M.L., et al. (1976) Gastroenterology 71,965-970. J. (1972) Rev. Can. Biol. x,253-257. Mass, C., Morisset, J., Dunnigan, Bonting, S.L. (1972) Biochim, et Biophys. Rutten,W.J..DePont, J.J.H.H.M., Acta z,201-213. Gardner, J.D. (1975) in Gastrointestinal Klaeveman, H.L., Conlon, T.P., Ed.) p 321-344, University of Texas Press, Austin, Hormones (Thompson,J.C., and London B$*'G A (1960)'Anal Biochem 1 279 Gilmin,'A:G. (1970) P&c. Natl.'AFid, Sci. 67, 305-312. Lowry, O.H., Rosebrough, N.J., Farr, A.L., et al. (1951) J. Biol. Chem.
m,265-275. 12. Corbin, J.D., 13. 14. :;: 17. 18. 19. 20.
Park, C.R. (1973) J. Biol. Chem. 248, Soderling, T.R., 1813-1821. Keely, S.L.,Soderling, T.R., et al. (1975) in Advances in Corbin, J.D., Cyclic Nucleotide Research (Drummond,G.I., Greengard, P., Robison, ,G.A. Eds.) Vol. 5, p 265-279 Raven Press, New York. Kimberg, D.V. (1974) Gastroenterology 67, 1023-1064. Tompkins, R.K., Kuchenbecker, S.L. (1973) J. Surg. Res. x,172-176. G. (1974) Life Sci. I& 631-639. Heisler, S., Grondin, G., Forget, Deschodt-Lanckman, M., Robberecht, P., DeNeef, P., et al. (1975) Gastroenterology 68, 318-325. Lemon, M.J.C., Bhoola, K.D. (1975) Biochim. et Biophys. Acta 385,101-113. Domschke, S., Konturek, S.J.,Domschke, W., et al. (1975) Proc. Sot. Exp. Biol. Med. 150, 773-779. Domschke, S., Domschke, W.,Konturek, S., et al. (1976) Gastroenterology
z,533-536.
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95, No.
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BIOCHEMICAL
AND
BlOPHYSlCAL
RESEARCH
21. Case,R.M.,Johnson, M., Scratchert, T., et al. (1972) J. 669-684. 22. Marois, C., Morisset, J., Dunnigan, J. (1972) Rev. Can. 23. Rutten, W.J., DePont, J.J.H.H.M., Bonting, S.L. (1972) Acta =,201-213. 24. Kempen, H.J.M., DePont, J.J.H.H.M., Bonting, S.L. (1974) Biophys. Acta 370, 573-584 25. VanLeemput-Coutrez, M., Camus, J., Christophe, J. (1973) Res. Commun. 54, 182-190. G. (1957) 26. Cenatiempo, Y., Margeat, P., Marchis-Mauren, 865-873. J. (1975) Biochem. 27. Lambert, M., Camus, J., Christophe, 1755-1758. 28. Jensen, R.T.,Gardner, J.D. (1978) Gastroenterology 75,
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COMMUNICATIONS
Physiol.
223,
Biol. ~,253-257. Biochim. et Biophys. Biochim.
et
Biochem.
Biophys.
Biochimie,
57,
Pharmacol.
24,
806-817.