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The effect of temperature on the activity of the adenylate cyclase system of liver plasma membranes
Vol. 80, No. 3, 1978
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Pages 609-615
February 14, 1978
THE
EFFECT OF TEMPERATURE ON THE ACTIVITY
OF THE ADENYLATE
CYCLASE SYSTEM OF LIVER PLASMA MEMBRANES J. Antonio Biochemistry
Pliego*
Department,
Avanzados
de1 Instituto
Received
November 4,1977
and Boanerges Centro
PolitGcnico
Rubalcava'
de Investigaci6n
National,
P.O.
y de Estudios
Box 14-740,
Mexico
14, D.F.
SUMMARY The rat liver adenylate cyclase system shows a discontinuity in the Arrhenius plots at 20°C in the nonstimulated activity (basal) with activation energies of 16 and 28 Kcal/mole. The discontinuity disappears when the enzyme is stimulated either by glucagon, sodium fluoride, 5'guanylyl-imidodiphosphate or glucagon plus 5'guanylyl-imidodiphosphate and the energy of activation was the same with all the compounds tested. If the activator was initially in contact with the membranes at 0°C the energy of activation was similar to that observed below the break (26 Kcal/mole) but it changed to that above the break if the compound contacted the membranes at temperatures above the break (22-24°C). We discuss the possibility of two different conformations of the enzyme; both conformations can be "frozen" by any of the compounds tested, "isolating" the enzyme from any subsequent physical change of the membrane due to temperature. A model
has been proposed
In such a model, proteins liquid
the phospholipids
it
is
and the structure
phase
in which
the
operate
independently
thought rather
proteins
properties
system it
that than
membranes
their
is an intrinsic
There
activity effect
of the
several
cations
adenylate
is due to actions
on the enzyme lose
are
component
by the lipids
to be influenced
of the membrane. on the
although
(1).
globular but a
influenced
of the lipids.
cyclase expect
membrane
in a bilayer
It is not a rigid
of hormones
dispersed
arranged
plasma
phase.
protein
membrane
of the
in the lipid
we would
effect
are
structure
immersed
The adenylate
other
the
are
by the physical
therefore
for
the hormonal
itself.
It
response
cyclase on the
of membranes just
that
like
structure
retain
(2,3),
and
detergent
the ability
*Fellow of CONACYT Mexico. Presented as partial fullfilment for at Centro de Investigaci6n y de Estudios Avanzados de1 Instituto National. -!-To whom correspondence should be addressed.
the
of the
has been shown that but
any
influence
system
and
to re-
M. SC. degree Polit6cnico
OOO6-291X/78/0803-9609$01.0010
609
Copyright 0 1978 by Academic Press. Inc. All rights of reproduction in any form reserved.
BIOCHEMICAL
Vol. 80, No. 3, 1978
act
to the
specific dence
lipids that
affect ship
fluoride
on the
acidic
the
rat
(4-8).
liver
of this
of these
enzyme system.
studies
the discontinuities
enzyme activities and separations)
relationship
with
The present
ious
(8);
lipids
adenylate
changes study
and the
activity
with
either
to
relationof the
that
controls
the ac-
in the Arrhenius
plots
of mem-
phase
changes
with
lipid
to establish
activation
effect
a clear
binding
to a site
and have intended
the
of
and nucleotides
we showed
have been correlated
describes
the participation
glucagon
also
in the Arrhenius
cyclase
suggest
for
or of nucleotides
(transitions
membrane
required
cyclase
RESEARCH COMMUNICATIONS
We have presented sOmeevi-
(8-11).
regulatory
In several bound
are
adenylate
residue
studies
action
phospholipids
histidine
tivity
Previous
hormonal
between the presence
glucagon
brane
ion
AND BIOPHYSICAL
a physiological
energy
of temperature
and without
the
(12-15). on the
stimulation
rat
liver of var-
compounds. MATERIALS
AND METHODS
Glucagon was supplied as a gift by Lilly.[a-32P]ATP, Gpp(NH)p' and cyclic AMP were supplied by the International Chemical and Nuclear Corporation Creatine phosphate and creatine and used without any further purification. phosphokinase were purchased from Sigma Chemical Co. All other reagents were of analytical grade. Partially purified plasma membranes from rat liver (male Wistar rats) were prepared according to Neville's procedure (16) with a modification described by Pohl et al. (17), and frozen and stored in liquid nitrogen. For further use the membranes were suspended in 20 mM Tris-HCl, pH 7.5. Adenylate cyclase activity was measured by the method described by Salomon, Londos and Rodbell (18). Unless specified otherwise, the assay medium contained 3.2 mM 25 mM Tris-HCl pH 7.5,1 mM cyclic [CP P]ATP (20-40 cpm/pmole), 5 mM MgC12, AMP and an ATP regenerating system consisting of 20 mM creatine phosphate and 100 U/ml creatine phosphokinase. Either glucagon, sodium fluoride, Gpp(NH)p or Glucagon plus Gpp(NH)p was added to stimulate the enzymatic activity. Incubations were carried out for ten minutes at the temperature indicated. Unless stated otherwise, the reaction was initiated by the addition of the membranes which were measured by the procedure of to give 30-40 micrograms of proteins, Lowry et al. (19) using bovine serum albumin as standard. The slopes of the Arrhenmots and the existence and locations of break points were determined by linear regression analysis, and the activation energies of the basal and stimulated activities were compared to each other by the Student test. RESULTS AND DISCUSSION Under
the conditions
=The abbreviations AMP, adenosine
of the assay
used are: Gpp(NH)p, 3':5'monophosphate.
for
basal
and stimulated
5'guanylyl-imidodiphosphate;
610
activities Cyclic
BIOCHEMICAL
Vol. 80, No. 3, 1978
with
10w6M glucagon
cyclase the
activity
specific
(5,12).
and 10 mM sodium is
linear
activity
We were
AND BIOPHYSICAL
in time
fluoride, during
to measure
the
we found
that
the ten minutes
was of the same order
able
RESEARCH COMMUNICATIONS
of the
basal
adenylate
of incubation
values
activity
the
and
previously
reported
at temperatures
as
low
as 5°C. The temperature as shown in Fig. activity the
1, where
presents
activities Gpp(NH)p
ally
the
the break
by adding
stimulated performed
point described
activities
the membranes
already
the plot
of
or glucagon energy
to that
is essenti-
of the basal
activi-
I).
obtained
through
initiating
medium,
contained
the
activators,
activity
the
break
basal
change
the conformation
this
hypothesis,
that
the reac-
in the case of
and this
addition
was
these
conditions
between
similar
point
(Fig
2) (Table
To assure
that
this
experiments:
I5 minutes,
then
the break
I,
but
also
two different first, we added
we kept
found
energy for
of the
the basal
added
and then reaction
activity
under above
II).
to the
stabilizing
active
conformations,
the membranes
611
in
but keeping
15 minutes
not have a different
the activator
seems
point.
the above experiments,
Condition did
plot
the activator
22 and 24°C for
to that
reaction
to the temperature
activities
The activation
solution.
was very
on an enzyme with
below
of the Arrhenius
of the enzyme due to a change
we repeated
at temperatures
to the activator
for
similar
incubation
of a conformational
added
following
to the
fluoride
The activation
condition
of the basal
2O"C, whereas
sodium
and in the case of the stimulated
To test
tors
I,
plot
differently,
at 0°C.
seems to "freeze"
due only
and very
above were
the membranes
to be the result
the break
such a break.
(Table
In the case of the
the lipids
by glucagon,
each compound
activities
the Arrhenius
at approximately
either
do not present
same for
and stimulated
is seen that
a discontinuity
The results tion
the basal
it
stimulated
plus
ty below
affected
activation action
of the activa-
we performed
above
and returned
energy
20°C
the
(22-24'C)
the mixture
to an
BIOCHEMICAL
Vol. 80, No. 3, 1978
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
20 I 0
IO “C I Glucogon
+ GPP IN H jp
Fig. 1 Arrhenius plot of the adenylate cyclase activity (nmoles cyclic AMP/mg protein in ten minutes) Effect of 10 mM Sodium fluoride, lO-'jM glucagon and lO-'jM glucagon combined with 10-5M Gpp(NH)p. The membranes at 0°C were added to the incubation medium (see methods) containing the activators (Condition I). The different symbols for the basal activity indicate 3 different experiments with membranes frozen in liquid nitrogen one year ( D ) 6 months ( A ) and one week ( ) before the experiment.
l
ice bath
and at this
point
The activation
energy
basal
above the
tion
activity III-A
(Table
the substrate ice-bath; observed
Finally,
was,
substrate
break
point
is a control
an experiment
conditions
(Table
I,
in which
the
the activation below
was performed
612
to start
the reaction.
the same as in the case of the
membrane-activator
as we expected, the basal
was added
as we expected,
to the mixture
again, under
I)
the
Condition
The condi-
reaction
was started
which
had been kept
energy
the break that
III-B).
was similar
by adding in an to that
point.
probed
that
the
change
in
BIOCHEMICAL
Vol. 80, No. 3, 1978
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE
THE EFFECT OF VARIOUS
I
COMPOUNDS ON THE ENERGY OF ACTIVATION
OF A~ENYLATE COMPOUND ADDED
CONDITION
NONE (BASAL)
27.9
+ 2.5(12)
15.G
+ 0.98(11)*’
GLUCAGON
26.0
t 2.8(11)
FLUORIDE
25.5
GPP(NH)P
24.9
GLUCAGON+ GPP(NH)P
26.4
(Kcal/mol)
CYCLASE
I*
CONDITION
II*
CONDITION
III*
A
17.0
+ 0.73(10)
+ 1.2(E)
17.1
+ 1.6(6)
+ 2.0(4)
18.5
+ 0.12(3)
r 1.6(7)
18.5
T 0.91(5)
The results are expressed as mean + S. D. results that qave a determination coefficient The range of femperature studied was 10" l For definition of conditions I, II and ** The basal activity showed a change in
The figures in parentheses < 0.9 were discarded. - 30°C. III see the text.+ the slope at 19.7"0.99'.
the enzyme due to temperature
is
activator
15 minutes,
standed
at 23°C for
returned
to the
and the
experiments
(not
shown)
ice-bath
were
was similar
those
expected
(27 Kcal/mole)
and after
as described for
to that
the
number
that the
such a condition: observed
for
performed.
slowly was added The results
activation
basal
(1)
the
were
I.
the
the
without
activator
+ 0.63(3)
17.5
of experiments
time
in condition
17.7
(1)
the membranes
Once there,
performed
i 0.50(Z)
24.7 are
reversible:
temperature.
were
25.5
8
below
energy
the break
point. The Student dicative
that
III-A
and the
being
identical.
vation for
This animal
the
with
results
basal
all
the
of the
activation
data
of the experiments
of the activation
experiments
energy
The probability
energies
activity
test
done under
below
was also
energies conditions
20°C had a high high
done under
was in-
to be the conditions
I and
probability same for
II
of the acti-
and III-B
and
above 20°C. study
presents
shows that a biphasic
the adenylate behavior
cyclase
in the Arrhenius
613
enzyme from a homeothermic plots.
This
is not
The
Vol. 80, No.3,
BIOCHEMICAL
1978
A SODIUM 0 0
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
FLUORIDE
GPP(NHIP GLUCAGON
:
w
Fig. 2 Arrhenius plot of the adenylate cyclase activity (nmoles cyclic AMP/mg protein in ten minutes). Effect of 10 mM sodium fluoride, 10-6M glucagon, lo-'M Gpp(NH)p and 10-6M glucagon combined with lo-'M Gpp(NH)p. The plasma membranes were incubated at 23°C for 15 minutes and then were added to the medium (see methods) containing the activators (Condition II).
surprising
since
various
shown the same behavior a result
of a change
viscosity covalent
probes labeling
membrane (20).
enzymes
This
lipid
of the membrane
the features
of that
the changes
observed
behavior
in the membrane
of the membrane
change
in studies
lipid core
components
in the membrane
on the enzyme.
Although
614
already
has been usually phase (21)
(12-15,
20).
and some kind
(22)
could
help
and its
possible
all
the activators
published
have
interpreted
as
The use of of photoactive to elucidate relationship used here
with act
BIOCHEMICAL
Vol. 80, No. 3, 1978
at different energy,
but
tivation the
sites instead
energy;
components
subsequent
of the complex all this
physical
In conclusion, to cyclic
AMP with
to a conformational tion
of the
physical
(5,
23)
they
of them "stabilize" suggests
of the
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
system,
changes
and this
the adenylate two activation change state
activators
tested
are able
when added
to the membranes.
the
the existence
of the
of the
do not modify system
of a high
the activation
with
the very
cooperativity
"stabilization"
same acamong
isolates
it
from
lipids. cyclase
catalizes
energies.
It
is
enzyme possibly
of the membrane. to stabilize
Also,
the conversion proposed
that
as a result it
is
this
is
due
of a modifica-
proposed
the enzyme conformation
of ATP
that
the
they
find
REFERENCES 1. Singer, S. J., and Nicholson, G. L. (1972) Science 175, 720-728. 2. Wolff, J., Berens, S. C., and Jones, A. B. (1970) Biochem. Biophys. Res. Con-m. 39, 77-82. 3. Lefkowithz, R. J., Roth, J., and Pastan, I, (1970) Nature 228, 864-866. 4. Sutherland, E. W., Rall, T. W., and Menon, T. (1972) J. Biol. Chem. 327, 1220-1227. 5. Birnbaumer, L., Pohl, S. L., and Rodbell, M. (1971) J. Biol. Chem. 246, 1857-1860. 6. Wolff, J., and Jones, A. B. (1971) 3. Biol. Chem. 3939-3847. 7. Wolff., J. and Jones, A. B. (1970) Proc. Natl. Acad. Sci. USA 454-459. 8. Rubalcava, B., and Rodbell, M. (1973) J. Biol. Chem. 248, 3831-3837. 9. Pohl, S. L., Krans, H.M. J., Kozireff, V., Birnbaumer, L., and Rodbell, M. (1971) J. Biol. Chem. 246, 4447-4454. 10. Levey, G. S., (1971) Biochem. Biophys. Res. Connn. 43, 108-113. 11. Levey, G. S., (1971) 3. Biol. Chem. 246, 7405-7407. 12. Wynn-Williams, A. T., (1976) Biochem. J. 157, 279-281. 13. Kumamoto, J., Raison, J. K., and Lyons, J. M. (1971) J. Theoret. Biol. 31, 47-51. 14. Raison, J. K., Lyons, J. M., Mehlforn, R. J. and Keith, A. 0. (1971), J. Biol. Chem. 246, 4036-4040. 15. Wisniesky, B. J., Parkes, J. G., Huang, Y. O., and Fox, F. (1974) Proc. Nat1 Acad. Sci. USA 71, 4381-4385. 16. Neville, 0. R. (1968) Biochem. Biophys. Acta 154, 540-552. 17. Pohl, S. L., Birnbaumer, L., and Rodbell, M. (1971) J. Biol. Chem. 246, 1849-1856. 18. Salomon, Y., Londos, C., and Rodbell, M. (1974) Anal. Biochem. 58, 541-548. 19. Lowry, O.H., Rosenbrough, N.Y., Farr, A. L., and Randall, R. J. (1951) J. Biol. Chem. 193, 265-275. 20. Raison, J. K., (1973) Bioenergetics 4, 285-309. 21. Rudy, B., and Gitler, C. (1972) Biochem., Biophys. Acta 228, 231-236. 22. Klip, A. and Gitler, C. (1974) Biochem. Biophys. Res. Comm. 60, 1155-1162. 23. Birnbaumer, L. (1973) Biochem. Biophys. Acta 300, 129-158.
615
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Pages 609-615
February 14, 1978
THE
EFFECT OF TEMPERATURE ON THE ACTIVITY
OF THE ADENYLATE
CYCLASE SYSTEM OF LIVER PLASMA MEMBRANES J. Antonio Biochemistry
Pliego*
Department,
Avanzados
de1 Instituto
Received
November 4,1977
and Boanerges Centro
PolitGcnico
Rubalcava'
de Investigaci6n
National,
P.O.
y de Estudios
Box 14-740,
Mexico
14, D.F.
SUMMARY The rat liver adenylate cyclase system shows a discontinuity in the Arrhenius plots at 20°C in the nonstimulated activity (basal) with activation energies of 16 and 28 Kcal/mole. The discontinuity disappears when the enzyme is stimulated either by glucagon, sodium fluoride, 5'guanylyl-imidodiphosphate or glucagon plus 5'guanylyl-imidodiphosphate and the energy of activation was the same with all the compounds tested. If the activator was initially in contact with the membranes at 0°C the energy of activation was similar to that observed below the break (26 Kcal/mole) but it changed to that above the break if the compound contacted the membranes at temperatures above the break (22-24°C). We discuss the possibility of two different conformations of the enzyme; both conformations can be "frozen" by any of the compounds tested, "isolating" the enzyme from any subsequent physical change of the membrane due to temperature. A model
has been proposed
In such a model, proteins liquid
the phospholipids
it
is
and the structure
phase
in which
the
operate
independently
thought rather
proteins
properties
system it
that than
membranes
their
is an intrinsic
There
activity effect
of the
several
cations
adenylate
is due to actions
on the enzyme lose
are
component
by the lipids
to be influenced
of the membrane. on the
although
(1).
globular but a
influenced
of the lipids.
cyclase expect
membrane
in a bilayer
It is not a rigid
of hormones
dispersed
arranged
plasma
phase.
protein
membrane
of the
in the lipid
we would
effect
are
structure
immersed
The adenylate
other
the
are
by the physical
therefore
for
the hormonal
itself.
It
response
cyclase on the
of membranes just
that
like
structure
retain
(2,3),
and
detergent
the ability
*Fellow of CONACYT Mexico. Presented as partial fullfilment for at Centro de Investigaci6n y de Estudios Avanzados de1 Instituto National. -!-To whom correspondence should be addressed.
the
of the
has been shown that but
any
influence
system
and
to re-
M. SC. degree Polit6cnico
OOO6-291X/78/0803-9609$01.0010
609
Copyright 0 1978 by Academic Press. Inc. All rights of reproduction in any form reserved.
BIOCHEMICAL
Vol. 80, No. 3, 1978
act
to the
specific dence
lipids that
affect ship
fluoride
on the
acidic
the
rat
(4-8).
liver
of this
of these
enzyme system.
studies
the discontinuities
enzyme activities and separations)
relationship
with
The present
ious
(8);
lipids
adenylate
changes study
and the
activity
with
either
to
relationof the
that
controls
the ac-
in the Arrhenius
plots
of mem-
phase
changes
with
lipid
to establish
activation
effect
a clear
binding
to a site
and have intended
the
of
and nucleotides
we showed
have been correlated
describes
the participation
glucagon
also
in the Arrhenius
cyclase
suggest
for
or of nucleotides
(transitions
membrane
required
cyclase
RESEARCH COMMUNICATIONS
We have presented sOmeevi-
(8-11).
regulatory
In several bound
are
adenylate
residue
studies
action
phospholipids
histidine
tivity
Previous
hormonal
between the presence
glucagon
brane
ion
AND BIOPHYSICAL
a physiological
energy
of temperature
and without
the
(12-15). on the
stimulation
rat
liver of var-
compounds. MATERIALS
AND METHODS
Glucagon was supplied as a gift by Lilly.[a-32P]ATP, Gpp(NH)p' and cyclic AMP were supplied by the International Chemical and Nuclear Corporation Creatine phosphate and creatine and used without any further purification. phosphokinase were purchased from Sigma Chemical Co. All other reagents were of analytical grade. Partially purified plasma membranes from rat liver (male Wistar rats) were prepared according to Neville's procedure (16) with a modification described by Pohl et al. (17), and frozen and stored in liquid nitrogen. For further use the membranes were suspended in 20 mM Tris-HCl, pH 7.5. Adenylate cyclase activity was measured by the method described by Salomon, Londos and Rodbell (18). Unless specified otherwise, the assay medium contained 3.2 mM 25 mM Tris-HCl pH 7.5,1 mM cyclic [CP P]ATP (20-40 cpm/pmole), 5 mM MgC12, AMP and an ATP regenerating system consisting of 20 mM creatine phosphate and 100 U/ml creatine phosphokinase. Either glucagon, sodium fluoride, Gpp(NH)p or Glucagon plus Gpp(NH)p was added to stimulate the enzymatic activity. Incubations were carried out for ten minutes at the temperature indicated. Unless stated otherwise, the reaction was initiated by the addition of the membranes which were measured by the procedure of to give 30-40 micrograms of proteins, Lowry et al. (19) using bovine serum albumin as standard. The slopes of the Arrhenmots and the existence and locations of break points were determined by linear regression analysis, and the activation energies of the basal and stimulated activities were compared to each other by the Student test. RESULTS AND DISCUSSION Under
the conditions
=The abbreviations AMP, adenosine
of the assay
used are: Gpp(NH)p, 3':5'monophosphate.
for
basal
and stimulated
5'guanylyl-imidodiphosphate;
610
activities Cyclic
BIOCHEMICAL
Vol. 80, No. 3, 1978
with
10w6M glucagon
cyclase the
activity
specific
(5,12).
and 10 mM sodium is
linear
activity
We were
AND BIOPHYSICAL
in time
fluoride, during
to measure
the
we found
that
the ten minutes
was of the same order
able
RESEARCH COMMUNICATIONS
of the
basal
adenylate
of incubation
values
activity
the
and
previously
reported
at temperatures
as
low
as 5°C. The temperature as shown in Fig. activity the
1, where
presents
activities Gpp(NH)p
ally
the
the break
by adding
stimulated performed
point described
activities
the membranes
already
the plot
of
or glucagon energy
to that
is essenti-
of the basal
activi-
I).
obtained
through
initiating
medium,
contained
the
activators,
activity
the
break
basal
change
the conformation
this
hypothesis,
that
the reac-
in the case of
and this
addition
was
these
conditions
between
similar
point
(Fig
2) (Table
To assure
that
this
experiments:
I5 minutes,
then
the break
I,
but
also
two different first, we added
we kept
found
energy for
of the
the basal
added
and then reaction
activity
under above
II).
to the
stabilizing
active
conformations,
the membranes
611
in
but keeping
15 minutes
not have a different
the activator
seems
point.
the above experiments,
Condition did
plot
the activator
22 and 24°C for
to that
reaction
to the temperature
activities
The activation
solution.
was very
on an enzyme with
below
of the Arrhenius
of the enzyme due to a change
we repeated
at temperatures
to the activator
for
similar
incubation
of a conformational
added
following
to the
fluoride
The activation
condition
of the basal
2O"C, whereas
sodium
and in the case of the stimulated
To test
tors
I,
plot
differently,
at 0°C.
seems to "freeze"
due only
and very
above were
the membranes
to be the result
the break
such a break.
(Table
In the case of the
the lipids
by glucagon,
each compound
activities
the Arrhenius
at approximately
either
do not present
same for
and stimulated
is seen that
a discontinuity
The results tion
the basal
it
stimulated
plus
ty below
affected
activation action
of the activa-
we performed
above
and returned
energy
20°C
the
(22-24'C)
the mixture
to an
BIOCHEMICAL
Vol. 80, No. 3, 1978
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
20 I 0
IO “C I Glucogon
+ GPP IN H jp
Fig. 1 Arrhenius plot of the adenylate cyclase activity (nmoles cyclic AMP/mg protein in ten minutes) Effect of 10 mM Sodium fluoride, lO-'jM glucagon and lO-'jM glucagon combined with 10-5M Gpp(NH)p. The membranes at 0°C were added to the incubation medium (see methods) containing the activators (Condition I). The different symbols for the basal activity indicate 3 different experiments with membranes frozen in liquid nitrogen one year ( D ) 6 months ( A ) and one week ( ) before the experiment.
l
ice bath
and at this
point
The activation
energy
basal
above the
tion
activity III-A
(Table
the substrate ice-bath; observed
Finally,
was,
substrate
break
point
is a control
an experiment
conditions
(Table
I,
in which
the
the activation below
was performed
612
to start
the reaction.
the same as in the case of the
membrane-activator
as we expected, the basal
was added
as we expected,
to the mixture
again, under
I)
the
Condition
The condi-
reaction
was started
which
had been kept
energy
the break that
III-B).
was similar
by adding in an to that
point.
probed
that
the
change
in
BIOCHEMICAL
Vol. 80, No. 3, 1978
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE
THE EFFECT OF VARIOUS
I
COMPOUNDS ON THE ENERGY OF ACTIVATION
OF A~ENYLATE COMPOUND ADDED
CONDITION
NONE (BASAL)
27.9
+ 2.5(12)
15.G
+ 0.98(11)*’
GLUCAGON
26.0
t 2.8(11)
FLUORIDE
25.5
GPP(NH)P
24.9
GLUCAGON+ GPP(NH)P
26.4
(Kcal/mol)
CYCLASE
I*
CONDITION
II*
CONDITION
III*
A
17.0
+ 0.73(10)
+ 1.2(E)
17.1
+ 1.6(6)
+ 2.0(4)
18.5
+ 0.12(3)
r 1.6(7)
18.5
T 0.91(5)
The results are expressed as mean + S. D. results that qave a determination coefficient The range of femperature studied was 10" l For definition of conditions I, II and ** The basal activity showed a change in
The figures in parentheses < 0.9 were discarded. - 30°C. III see the text.+ the slope at 19.7"0.99'.
the enzyme due to temperature
is
activator
15 minutes,
standed
at 23°C for
returned
to the
and the
experiments
(not
shown)
ice-bath
were
was similar
those
expected
(27 Kcal/mole)
and after
as described for
to that
the
number
that the
such a condition: observed
for
performed.
slowly was added The results
activation
basal
(1)
the
were
I.
the
the
without
activator
+ 0.63(3)
17.5
of experiments
time
in condition
17.7
(1)
the membranes
Once there,
performed
i 0.50(Z)
24.7 are
reversible:
temperature.
were
25.5
8
below
energy
the break
point. The Student dicative
that
III-A
and the
being
identical.
vation for
This animal
the
with
results
basal
all
the
of the
activation
data
of the experiments
of the activation
experiments
energy
The probability
energies
activity
test
done under
below
was also
energies conditions
20°C had a high high
done under
was in-
to be the conditions
I and
probability same for
II
of the acti-
and III-B
and
above 20°C. study
presents
shows that a biphasic
the adenylate behavior
cyclase
in the Arrhenius
613
enzyme from a homeothermic plots.
This
is not
The
Vol. 80, No.3,
BIOCHEMICAL
1978
A SODIUM 0 0
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
FLUORIDE
GPP(NHIP GLUCAGON
:
w
Fig. 2 Arrhenius plot of the adenylate cyclase activity (nmoles cyclic AMP/mg protein in ten minutes). Effect of 10 mM sodium fluoride, 10-6M glucagon, lo-'M Gpp(NH)p and 10-6M glucagon combined with lo-'M Gpp(NH)p. The plasma membranes were incubated at 23°C for 15 minutes and then were added to the medium (see methods) containing the activators (Condition II).
surprising
since
various
shown the same behavior a result
of a change
viscosity covalent
probes labeling
membrane (20).
enzymes
This
lipid
of the membrane
the features
of that
the changes
observed
behavior
in the membrane
of the membrane
change
in studies
lipid core
components
in the membrane
on the enzyme.
Although
614
already
has been usually phase (21)
(12-15,
20).
and some kind
(22)
could
help
and its
possible
all
the activators
published
have
interpreted
as
The use of of photoactive to elucidate relationship used here
with act
BIOCHEMICAL
Vol. 80, No. 3, 1978
at different energy,
but
tivation the
sites instead
energy;
components
subsequent
of the complex all this
physical
In conclusion, to cyclic
AMP with
to a conformational tion
of the
physical
(5,
23)
they
of them "stabilize" suggests
of the
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
system,
changes
and this
the adenylate two activation change state
activators
tested
are able
when added
to the membranes.
the
the existence
of the
of the
do not modify system
of a high
the activation
with
the very
cooperativity
"stabilization"
same acamong
isolates
it
from
lipids. cyclase
catalizes
energies.
It
is
enzyme possibly
of the membrane. to stabilize
Also,
the conversion proposed
that
as a result it
is
this
is
due
of a modifica-
proposed
the enzyme conformation
of ATP
that
the
they
find
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