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Cyclocreatine phosphate as a substitute for creatine phosphate in vertebrate tissues. Energetic considerations
BIOCHEMICAL
Vol. 74, No. 1, 1977
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
CYCLOCREATINE PHOSPHATE AS A SUBSTI!I'UTE FOR CREATINE PHOSPHATE IN VERTEBRATE TISSUES.
ENERGETIC CONSIDERATIONS
Thomas M. Annesley Department
of Biochemistry,
Received
and James B. Walker
William
Marsh
Rice
University,
Houston,
TX 77001
November 2,1976 SUMMARY
The measured equilibrium constant ;f the reaction, P-creatine*+ cyclocreatine + creatine + P-cyclocreatine catalyzed by creatine kinase in the presence of a trace of MgATP, is 26 at $'O. P-Cyclocreatine has a V,,, 0.6% that of P-creatine and a Km of 3.7 mM, vs. 2.8 rnM for P-creatine, with chick breast muscle creatine kinase at pH 7.0. These results suggest that the high ratio of P-cyclocreatine/cyclocreatine (ea. 45) previously observed in breast muscle of cyclocreatine-fed chicks, compared to the much lower ratio of P-creatine/creatine (ca. 2) in ' the same tissue, primarily reflects free energy relationships between the synthetic and natural phosphagens. Rowley creatine is
et al.
(I)
have synthesized
and shown that
an excellent
Griffiths
(2)
to 60 mM P-cyclocreatine authors
suggested
cyclocreatine much lower
(ca. ratio
equilibrium
for
creatine
found
that
in the
(2)
that
45)
the
conditions
for
In this approach in the
breast
paper
we report
was to determine presence
Cyclocreatine kinase was purified
of creatine
(ca.
Reaction
1
e
MgADPl-
concentration
in support
the apparent
ratio
equilibrium
and a trace
1).
muscle.
compared
primarily
These
with
the
reflected
near-
2-
(1)
+ H+
+ P-cyclocreatine2kinase
in skeletal
of this
suggestion.
constant amount
up
of P-cyclocreatine/
+ P-cyclocreatine
of creatine
of
accumulated
of breast
muscle,
2),
+ creatine MgATP)
evidence
kinase
(Reaction chicks
water high
in chick
+ cyclocreatine high
in vitro
sarcoplasmic
(tr. of the
analogs
(cyclocreatine)
cyclocreatine-fed
unexpectedly
observed
+ MgATP*-
P-Creatine2in view
kinase
of P-creatinelcreatine
Cyclocreatine
of potential
l-carboxymethyl-2-iminoimidazolidine
substrate
and Walker
a number
(2) muscle. Our
of Reaction
2
of MgATP.
MATERIALS AND METHODS was synthesized as described elsewhere (2). Creatine from chicken breast muscle (3) to a S. A. of 250 Clmol/
Copyright 0 1977 by Academic Press, Inc. All rights of reproduction in any form reserved.
185
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
I 0.5 ATP, MM
,
RESEARCH COMMUNICATIONS
I I .o
Fig. 1. Curve showing that attainment of the equilibrium of Reaction 2, catalyzed by creatine kinase, requires ATP. Initial conditions were identical to the first experiment of Table I. After incubation for 15 min, the creatine formed from P-creatine + cyclocreatine was determined colorimetritally. The equilibrium concentration would be 33.5 mM creatine.
min/mg protein at 300 and pH 9.0, assayed by the pH-stat method. Only one band was observed on SDS gels. Enzyme was stored at ho in 50 mM Tris.HCl, pH 8.0, and 14 mM mercaptoethanol. Calorimetric assays for the reactants of Reaction 2 were performed as described for the same four compounds in chick breast muscle (2). P-Cyclocreatine and P-creatine concentrations were obtained by substracting concentrations of cyclocreatine and creatine from the corresponding total values obtained after heating aliquots at 650 in 0.2 M perchloric acid for 15 min (P-creatine) and 45 min (P-cyclocreatine). Keq of Reaction 2 was measured after incubation of reactants for up to 8 hours at volume containing: Mg acetate, 2 mM; ATP, 1 mM; creatine 37O in 5 ml total kinase, 3 mg; and 50 mM of either triethanolamine.HCl, pH 7.0, or Na glycine, pH 9.0. Kinetic constants for creatine kinase were determined by coupled enzyme assays (a) in the forward direction by measuring ADP formed by NADH disappearance (4), and (b) in the reverse direction by measuring ATP formed by NADPH appearance (5). The reverse direction was also assayed by colorimetric determination of cyclocreatine or creatine formed (2). Initially cyclocreatine was chemically phosphorylated in this laboratory (by G. R. Griffiths) with Poll and NaOH and the product purified by column chromatography on Dowex-l(HCqactive isomer to be formed. 3 . We found only the enzymically for large scale synthesis (G.L. Kenyon, However, the use of LiOH is preferable personal communication). Cyclocreatine (45 g) was dissolved in 275 ml of 3 M LiOH and cooled to Oo with a dry ice-ethanol bath during the stepwise addition over 2 hours of a total of I20 ml of PoCl3 and 1000 ml of 3 M LiOH. The LiOH was added at intervals to keep the pH above 13. After 2.3 hours, the Li3PO4 and the supernatant solution was adjusted to pH was removed by filtration, 7.6 with 5 N HCl; 5 volumes of 95% ethanol were then added. The next day the fine precipitate was removed by filtration. The solution was cooled to -100 for 12 hours, then returned to room temperature to allow formation of crystals, which were filtered, washed with cold water and cold ethanol, and dried in a vacuum over P2O5. Yield: 25 g. The product was recsystallized from waterethanol, washed, dried, and stored at -100. The dilithium salt: (a) has an IR spectrum like that reported by Rowley et al. (1) for the enzymic product; (b) consists of only one active isomer as determined by coupled enzyme assay (5); (c) is hydrolyzed to cyclocreatine after 45 min at 650 in 0.2 M perchlo-
186
Vol. 74, No. 1, 1977
BIOCHEMICAL
TABIE I of Equilibrium Constant
Determination Conditions
AND BIOPHYSICAL RESEARCH COMMUNICATiONS
P-Creatine
Cyclocreatine
of Reaction
Creatine
2
P-Cyclocreatine
Keq
Initial Final
40 6
40 7
0 31
0 32
23.6
Initial Final
;
:
40 30
40 36
25.7
Initial Final
35 11
35 13
35 59
35 60
24.8
Initial Final
50 11
50 10
20 54
42”
20.6
Initial Final
5 5
5 5
25 27
25 27
29.2
bation
Concentrations (mM) of reactants for 6 to 8 hours at 370.
are
given
at 0 time
and after
incu-
ric acid (2); and (d) has pK,'s of approximately 3.1, 4.5, and 10.7. The active isomer is now known to be the 3-phosphono, rather than the 2-phosphono (l), derivative from X-ray crystallographic analysis (G. N. Phillips and F. A. Quiocho, in preparation)(cf. unpublished data cited in (6)).
Equilibration tine
kinase
provide tine
of the but
also
additional from
was selected
for
length
chick
MgADP),
against
breast
without
2 requires
as shown in Fig.
a double
muscle.
Keq determinations of time
RESULTS in Reaction
reactants
MgATP (or evidence
kinase
venient
four
displacement
An ATP (or in order
markedly
not
1. These
only results
mechanism
ADP) concentration
to achieve
perturbing
the
trea-
for
crea-
of 1 mM
equilibrium
in a con-
equilibrium
values
obtained. Table
I summarizes
five
separate
tions
of the
experiments four
was substituted We observed in the
the
physiological
data
at pH 7.0,
employing
reactants. for
that,
equilibrium
ATP, the like
The average average
P-creatine, range,
SO
Gq
for
value
Reaction different for
Gq was 28.4.
initial
from concentra-
Qq was 24.8.
When ADP
At pH 9.0 the
hq
none of the
pI&'s
of Reaction
2 should
187
2 obtained
was 25.7.
of P-cyclocreatine be pH-independent
occur
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
24
RESEARCH COMMUNICATIONS
-
02 I/
P-CREATINE
, u~-l
I/
0.4
0.6
P-CYCLOCREATINE
, MM-’
Fig. 2. Double-reciprocal kinetic plots for the reverse reaction catalyzed by chick breast muscle creatine kinase at pH 7.0 and 370. Incubation mixtures contained 37 mM Mg acetate, 11 mM ADP, and 29 mM triethanolamine.HCl, pH 7.0. P-Cyclocreatine: rC, = 3.7 mM; V, P-Creatine: & = 2.8 mM; V,,, =
over
a broad
range.
The overall
ATP or ADP and at pH 7.0 Kinetic muscle
data
creatine
3.7 mM for creatine
coupled
that
for
creatine
with
vided
chick
kinetic
parameters
catalyzed
reactants
by creatine
has provided
gives
the
kinase
(8)
1 obtained
corresponding
reaction
a value
of 26,
for
in agreement
188
2).
(cf.
from the
0.7$
by
of 55 m&f for
45%that
cyclofor
Substitution
relationships
when cyclocreatine on the
of 3.6 mM for
assayed
7).
of for
the
or creatine
I&q observed Haldane
with
creatine
with
the measured
of
ob-
P-cyclocreatine
a G
Haldane
Values
G's
cyclocreatine
kinase
check
Reaction
P-cyclo-
reaction,
indicated
respective
an independent
of Keq for
by Keq for
the
creatine
and a Vmax for
for
forward
and a V,,,
muscle into
and V,,
the
a &
and 37O were
7.0
breast
indicated
and 370 (Fig.
and 37O (4),
creatine
breast
for
by chick
method,
P-creatine
P-creatine, data
SD.
calorimetric
(5) at pH
of Keq, with
1 catalyzed
at pH 7.0
at pH 7.0
vs. 20 mM for
2. The ratio
P-creatine
kinetic
2 4.7
2.8 mM for
and 3.2 mM for
P-creatine.
substrates
by the
enzyme assay
enzyme assay
reaction
of Reaction
vs.
creatine
these
reverse
P-cyclocreatine
by coupled
for
was 25.8
assayed
P-cyclocreatine that
the
or 9.0,
kinase,
0.6%
tained
for
of 16 determinations
average
for
equation
and P-creatine Keq for
are
Reaction dias Reac-
BIOCHEMICAL
Vol. 74, No. 1, 1977
tion
2. In this
calculation
Mg,ATP and MgADP are
the
similar
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
assumptions
in both
were
made that
the
Km's for
reactions.
DISCUSSION This
work
thetic
was performed
phosphagen
difficult
from both
to determine
energy
of the
of P-cyclocreatine
relative
to ATP,
numerous
other
equilibria
Additional
would
(cf.
equilibrium fed range
10,ll).
(2),
is
thetic
lLq
for
relatively
natural
phosphagen
higher
than
resting
breast
by the
free
muscle
energy
relationships
For example, creatine larger
when
during total
reservoir
it
energy
pH over
the
rapid
growth,
to similar
cells
I)
less
physiological
nucleotides.
indicates
that free
of hydrolysis
(2)
The
this
energy
only
thus
2, without
of substitution
synthan
the
slightly in
can be explained
invoking
resting
of a major
by this prove
more stable
intracellu-
fast-twitch
during
of control 189
(2)
previously muscle
phosphate,
limited
portion
but a series
animals.
cells
the
interest. fed would
availability
of rapid
of the
synthetic
to be of considerable
in animals
that,
of high-energy
be kinetically
adenine
chicks
should
be predicted
an
of P-cyclocreatine/cyclocreatine
tissues
might
reservoir
would
compared
free
represents
muscular
equilibria.
consequences
of lower
2, which
reac-
of both
of Reaction
in vertebrate
of these
of cyclocreatine-
energy
ratio
ADP in pertinent
and during
chelated
of of
before
2 kcal/mol
a free
pK,'s
muscles
of cyclocreatine-fed
The physiological
phosphagen
i.e.
the
pH
breast
2 of 26 at 370 (Table
or additional
phosphagen
e.g.
involving
of ATP. The high
compartmentation
natural
independent
near
and unbound
Reaction
has approximately
pair,
that
tissues, hand,
at physiological
concentrations
in resting
constants
pair
Mg2'
is
free
such as determinations
equilibrium
other
attained
Reaction
phosphagen
if
in intact
On the
and dissociation
observed
lar
be involved
presumably
chicks
of free
It
1, and the
at pH's
complexities,
compartments,
to be estimated
involved
syn-
standpoints.
of Reaction
pH and concentrations
exercise
and kinetic
constant
intracellular
were
as a potential
equilibrium
MgATP and MgADP (8,g).
tants
P-cyclocreatine
the thermodynamic
the
of hydrolysis
because
to evaluate
cyclohave a of that
contractions,
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ACKNCklLEDGMENTS This work was supported by grant C-153 from the Robert A. Welch Foundation, Houston, Texas. T. M. A. is a Predoctoral Fellow of the Robert A. Welch Foundation.
REFERENCES 1. Rowley, G. L., Greenleaf, A. L., and Kenyon, G. L. (1971) J. Am,. Chem. Sot. 93, 5542-5551. 2. Griffiths, G. R., and Walker, J. B. (1976) J. Biol. Chem. 251, 2049-2054. 3. Dawson, D. M., and Eppenberger, H. M. (1970) Methods Enzymol. 17A, 995-1002. 4. Bernt, E., Bergmeyer, H. U., and Mollering, H. (1974) in Methods of Enzymatic Analysis (H. U. Bergmeyer, ed.) Vol. 4, pp. 1772-1776, Academic Press, New York. 5. Lamprecht, W., Stein, P., Heinz, F., and Weisser, H. (1974) in Methods of Enzymatic Analysis (H. U. Bergmeyer, ed.) Vol. 4, pp. 1777-1781, Academic Press, New York. 6. Kenyon, G. L., Struve, G. E., Kollman, P. A., and Moder, T. I. (1976) J. Am. Chem. Sot. 98, 3695-3699. 7. McLaughlin, A. C., Cohn, M., and Kenyon, G. L. (1972) J. Biol. Chem. 247, 4382-4388. 8. Nihei, T., Noda, L., and Morales, M. F. (1961) J. Biol. Chem. 236, 32033209. E. A. (1962) in The Enzymes, 2nd Ed., Vol. 6, 9. Kuby, S. A., and Noltmann, pp. 515-603, Academic Press, New York. T. W. (1974) J. Biol. Chem. 249, 5845-5850. 10. McGilvery, R. W., and Murray, E. (1975) Biochem. J. 152, 173-180. 11. Sahlin, K., Harris, R. C., and Hultman,
190
Vol. 74, No. 1, 1977
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
CYCLOCREATINE PHOSPHATE AS A SUBSTI!I'UTE FOR CREATINE PHOSPHATE IN VERTEBRATE TISSUES.
ENERGETIC CONSIDERATIONS
Thomas M. Annesley Department
of Biochemistry,
Received
and James B. Walker
William
Marsh
Rice
University,
Houston,
TX 77001
November 2,1976 SUMMARY
The measured equilibrium constant ;f the reaction, P-creatine*+ cyclocreatine + creatine + P-cyclocreatine catalyzed by creatine kinase in the presence of a trace of MgATP, is 26 at $'O. P-Cyclocreatine has a V,,, 0.6% that of P-creatine and a Km of 3.7 mM, vs. 2.8 rnM for P-creatine, with chick breast muscle creatine kinase at pH 7.0. These results suggest that the high ratio of P-cyclocreatine/cyclocreatine (ea. 45) previously observed in breast muscle of cyclocreatine-fed chicks, compared to the much lower ratio of P-creatine/creatine (ca. 2) in ' the same tissue, primarily reflects free energy relationships between the synthetic and natural phosphagens. Rowley creatine is
et al.
(I)
have synthesized
and shown that
an excellent
Griffiths
(2)
to 60 mM P-cyclocreatine authors
suggested
cyclocreatine much lower
(ca. ratio
equilibrium
for
creatine
found
that
in the
(2)
that
45)
the
conditions
for
In this approach in the
breast
paper
we report
was to determine presence
Cyclocreatine kinase was purified
of creatine
(ca.
Reaction
1
e
MgADPl-
concentration
in support
the apparent
ratio
equilibrium
and a trace
1).
muscle.
compared
primarily
These
with
the
reflected
near-
2-
(1)
+ H+
+ P-cyclocreatine2kinase
in skeletal
of this
suggestion.
constant amount
up
of P-cyclocreatine/
+ P-cyclocreatine
of creatine
of
accumulated
of breast
muscle,
2),
+ creatine MgATP)
evidence
kinase
(Reaction chicks
water high
in chick
+ cyclocreatine high
in vitro
sarcoplasmic
(tr. of the
analogs
(cyclocreatine)
cyclocreatine-fed
unexpectedly
observed
+ MgATP*-
P-Creatine2in view
kinase
of P-creatinelcreatine
Cyclocreatine
of potential
l-carboxymethyl-2-iminoimidazolidine
substrate
and Walker
a number
(2) muscle. Our
of Reaction
2
of MgATP.
MATERIALS AND METHODS was synthesized as described elsewhere (2). Creatine from chicken breast muscle (3) to a S. A. of 250 Clmol/
Copyright 0 1977 by Academic Press, Inc. All rights of reproduction in any form reserved.
185
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
I 0.5 ATP, MM
,
RESEARCH COMMUNICATIONS
I I .o
Fig. 1. Curve showing that attainment of the equilibrium of Reaction 2, catalyzed by creatine kinase, requires ATP. Initial conditions were identical to the first experiment of Table I. After incubation for 15 min, the creatine formed from P-creatine + cyclocreatine was determined colorimetritally. The equilibrium concentration would be 33.5 mM creatine.
min/mg protein at 300 and pH 9.0, assayed by the pH-stat method. Only one band was observed on SDS gels. Enzyme was stored at ho in 50 mM Tris.HCl, pH 8.0, and 14 mM mercaptoethanol. Calorimetric assays for the reactants of Reaction 2 were performed as described for the same four compounds in chick breast muscle (2). P-Cyclocreatine and P-creatine concentrations were obtained by substracting concentrations of cyclocreatine and creatine from the corresponding total values obtained after heating aliquots at 650 in 0.2 M perchloric acid for 15 min (P-creatine) and 45 min (P-cyclocreatine). Keq of Reaction 2 was measured after incubation of reactants for up to 8 hours at volume containing: Mg acetate, 2 mM; ATP, 1 mM; creatine 37O in 5 ml total kinase, 3 mg; and 50 mM of either triethanolamine.HCl, pH 7.0, or Na glycine, pH 9.0. Kinetic constants for creatine kinase were determined by coupled enzyme assays (a) in the forward direction by measuring ADP formed by NADH disappearance (4), and (b) in the reverse direction by measuring ATP formed by NADPH appearance (5). The reverse direction was also assayed by colorimetric determination of cyclocreatine or creatine formed (2). Initially cyclocreatine was chemically phosphorylated in this laboratory (by G. R. Griffiths) with Poll and NaOH and the product purified by column chromatography on Dowex-l(HCqactive isomer to be formed. 3 . We found only the enzymically for large scale synthesis (G.L. Kenyon, However, the use of LiOH is preferable personal communication). Cyclocreatine (45 g) was dissolved in 275 ml of 3 M LiOH and cooled to Oo with a dry ice-ethanol bath during the stepwise addition over 2 hours of a total of I20 ml of PoCl3 and 1000 ml of 3 M LiOH. The LiOH was added at intervals to keep the pH above 13. After 2.3 hours, the Li3PO4 and the supernatant solution was adjusted to pH was removed by filtration, 7.6 with 5 N HCl; 5 volumes of 95% ethanol were then added. The next day the fine precipitate was removed by filtration. The solution was cooled to -100 for 12 hours, then returned to room temperature to allow formation of crystals, which were filtered, washed with cold water and cold ethanol, and dried in a vacuum over P2O5. Yield: 25 g. The product was recsystallized from waterethanol, washed, dried, and stored at -100. The dilithium salt: (a) has an IR spectrum like that reported by Rowley et al. (1) for the enzymic product; (b) consists of only one active isomer as determined by coupled enzyme assay (5); (c) is hydrolyzed to cyclocreatine after 45 min at 650 in 0.2 M perchlo-
186
Vol. 74, No. 1, 1977
BIOCHEMICAL
TABIE I of Equilibrium Constant
Determination Conditions
AND BIOPHYSICAL RESEARCH COMMUNICATiONS
P-Creatine
Cyclocreatine
of Reaction
Creatine
2
P-Cyclocreatine
Keq
Initial Final
40 6
40 7
0 31
0 32
23.6
Initial Final
;
:
40 30
40 36
25.7
Initial Final
35 11
35 13
35 59
35 60
24.8
Initial Final
50 11
50 10
20 54
42”
20.6
Initial Final
5 5
5 5
25 27
25 27
29.2
bation
Concentrations (mM) of reactants for 6 to 8 hours at 370.
are
given
at 0 time
and after
incu-
ric acid (2); and (d) has pK,'s of approximately 3.1, 4.5, and 10.7. The active isomer is now known to be the 3-phosphono, rather than the 2-phosphono (l), derivative from X-ray crystallographic analysis (G. N. Phillips and F. A. Quiocho, in preparation)(cf. unpublished data cited in (6)).
Equilibration tine
kinase
provide tine
of the but
also
additional from
was selected
for
length
chick
MgADP),
against
breast
without
2 requires
as shown in Fig.
a double
muscle.
Keq determinations of time
RESULTS in Reaction
reactants
MgATP (or evidence
kinase
venient
four
displacement
An ATP (or in order
markedly
not
1. These
only results
mechanism
ADP) concentration
to achieve
perturbing
the
trea-
for
crea-
of 1 mM
equilibrium
in a con-
equilibrium
values
obtained. Table
I summarizes
five
separate
tions
of the
experiments four
was substituted We observed in the
the
physiological
data
at pH 7.0,
employing
reactants. for
that,
equilibrium
ATP, the like
The average average
P-creatine, range,
SO
Gq
for
value
Reaction different for
Gq was 28.4.
initial
from concentra-
Qq was 24.8.
When ADP
At pH 9.0 the
hq
none of the
pI&'s
of Reaction
2 should
187
2 obtained
was 25.7.
of P-cyclocreatine be pH-independent
occur
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
24
RESEARCH COMMUNICATIONS
-
02 I/
P-CREATINE
, u~-l
I/
0.4
0.6
P-CYCLOCREATINE
, MM-’
Fig. 2. Double-reciprocal kinetic plots for the reverse reaction catalyzed by chick breast muscle creatine kinase at pH 7.0 and 370. Incubation mixtures contained 37 mM Mg acetate, 11 mM ADP, and 29 mM triethanolamine.HCl, pH 7.0. P-Cyclocreatine: rC, = 3.7 mM; V, P-Creatine: & = 2.8 mM; V,,, =
over
a broad
range.
The overall
ATP or ADP and at pH 7.0 Kinetic muscle
data
creatine
3.7 mM for creatine
coupled
that
for
creatine
with
vided
chick
kinetic
parameters
catalyzed
reactants
by creatine
has provided
gives
the
kinase
(8)
1 obtained
corresponding
reaction
a value
of 26,
for
in agreement
188
2).
(cf.
from the
0.7$
by
of 55 m&f for
45%that
cyclofor
Substitution
relationships
when cyclocreatine on the
of 3.6 mM for
assayed
7).
of for
the
or creatine
I&q observed Haldane
with
creatine
with
the measured
of
ob-
P-cyclocreatine
a G
Haldane
Values
G's
cyclocreatine
kinase
check
Reaction
P-cyclo-
reaction,
indicated
respective
an independent
of Keq for
by Keq for
the
creatine
and a Vmax for
for
forward
and a V,,,
muscle into
and V,,
the
a &
and 37O were
7.0
breast
indicated
and 370 (Fig.
and 37O (4),
creatine
breast
for
by chick
method,
P-creatine
P-creatine, data
SD.
calorimetric
(5) at pH
of Keq, with
1 catalyzed
at pH 7.0
at pH 7.0
vs. 20 mM for
2. The ratio
P-creatine
kinetic
2 4.7
2.8 mM for
and 3.2 mM for
P-creatine.
substrates
by the
enzyme assay
enzyme assay
reaction
of Reaction
vs.
creatine
these
reverse
P-cyclocreatine
by coupled
for
was 25.8
assayed
P-cyclocreatine that
the
or 9.0,
kinase,
0.6%
tained
for
of 16 determinations
average
for
equation
and P-creatine Keq for
are
Reaction dias Reac-
BIOCHEMICAL
Vol. 74, No. 1, 1977
tion
2. In this
calculation
Mg,ATP and MgADP are
the
similar
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
assumptions
in both
were
made that
the
Km's for
reactions.
DISCUSSION This
work
thetic
was performed
phosphagen
difficult
from both
to determine
energy
of the
of P-cyclocreatine
relative
to ATP,
numerous
other
equilibria
Additional
would
(cf.
equilibrium fed range
10,ll).
(2),
is
thetic
lLq
for
relatively
natural
phosphagen
higher
than
resting
breast
by the
free
muscle
energy
relationships
For example, creatine larger
when
during total
reservoir
it
energy
pH over
the
rapid
growth,
to similar
cells
I)
less
physiological
nucleotides.
indicates
that free
of hydrolysis
(2)
The
this
energy
only
thus
2, without
of substitution
synthan
the
slightly in
can be explained
invoking
resting
of a major
by this prove
more stable
intracellu-
fast-twitch
during
of control 189
(2)
previously muscle
phosphate,
limited
portion
but a series
animals.
cells
the
interest. fed would
availability
of rapid
of the
synthetic
to be of considerable
in animals
that,
of high-energy
be kinetically
adenine
chicks
should
be predicted
an
of P-cyclocreatine/cyclocreatine
tissues
might
reservoir
would
compared
free
represents
muscular
equilibria.
consequences
of lower
2, which
reac-
of both
of Reaction
in vertebrate
of these
of cyclocreatine-
energy
ratio
ADP in pertinent
and during
chelated
of of
before
2 kcal/mol
a free
pK,'s
muscles
of cyclocreatine-fed
The physiological
phosphagen
i.e.
the
pH
breast
2 of 26 at 370 (Table
or additional
phosphagen
e.g.
involving
of ATP. The high
compartmentation
natural
independent
near
and unbound
Reaction
has approximately
pair,
that
tissues, hand,
at physiological
concentrations
in resting
constants
pair
Mg2'
is
free
such as determinations
equilibrium
other
attained
Reaction
phosphagen
if
in intact
On the
and dissociation
observed
lar
be involved
presumably
chicks
of free
It
1, and the
at pH's
complexities,
compartments,
to be estimated
involved
syn-
standpoints.
of Reaction
pH and concentrations
exercise
and kinetic
constant
intracellular
were
as a potential
equilibrium
MgATP and MgADP (8,g).
tants
P-cyclocreatine
the thermodynamic
the
of hydrolysis
because
to evaluate
cyclohave a of that
contractions,
Vol. 74, No. 1, 1977
BIOCHEMICAL
AND BIOPHYSICAL
RESEARCH COMMUNICATIONS
ACKNCklLEDGMENTS This work was supported by grant C-153 from the Robert A. Welch Foundation, Houston, Texas. T. M. A. is a Predoctoral Fellow of the Robert A. Welch Foundation.
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