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An in vitro increase in aspartyltranscarbamylase activity
Vol. 22, No. 6, 1966
AN IN
BIOCHEMICAL
lrITR0
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
INCREASE IN ASPARTYLTRANSCARBAMYLASE ACTIVITY* Raizada
MSU/AEC Plant
Received
Research
February
A number
tion
observed
with
have demonstrated
(cf.
Nisman
an increase
in a cell-free
When grown
of this
mutant
vitro
in ATCase activity
partially
Pathology
inhibited
of specific
is
cell-free
greater
by RNase, but
if
mutant
is
activity
of E. coli. about
and Schachman,
here
dependent
amino
12 per
cent
The in
1965).
on the presence
enzyme preparation
exogenous
communica-
(ATCase)
requiring
(Gerhart
enzymes
The following
ATCase contitutes
reported
+t and a dialyzed
in activity
1964).
from a uracil of uracil,
protein
The increase
and Pelmont,
amounts
of the soluble
of ATP, GTP and Mg
synthesis
of aspartyltranscarbamylase
system
on limiting
increase
and Plant
11, 1966
systems
deals
Singh
Laboratory and Department of Botany Michigan State University East Lansing, Michigan, 48823
of investigators
in cell-free
M.M.
of the mutant.
acids
are added
and is
not by puromycin. EXPERIMENTAL
The mutant containing all
limiting
subsequent
washed
was grown
aerobically
amounts
operations
in a standard
buffer
at 37'
of uracil performed
to early
log
phase
(8 pg/ml)'.
The cells
at 0 to 5'.
The harvested
containing
0.01 g potassium
in a medium
were cells
phosphateL
chilled
and
were pH 7.4,
*This investigation was supported in part by the U.S. Atomic Energy Commission, Contract No. AT(ll-l)-1338 and in part by research grant AM 05916 from the National Institutes of Health to Dr. R. S. Bandurski. 1 I thank Dr. .I. C. Gerhart for cating unpublished observations
providing regarding
the mutant of E. coZi and communisuitable growth conditions.
n
'Use of phosphate buffer during preparation tion medium more than doubled the increas.e observed with tris(hydroxymethyl)aminomethane
of the "enzymd'and in the incubain ATCase activity above that buffer at the same pH.
Vol. 22, No. 6, 1966
0.014
g magnesium
passage
through
centrifuged the
acetate
at 10,000
fluid
was dialyzed
a change
of buffer
with
"enzyme",
liquid
caused
centrifuged fluid natant.
stored
aliquots
the
Both
at -20'
after
of standard
enzyme was not
was raised
stored
to 0.03
About
quick
discarded,
and
The superfor
designated
quick
freezing
again
since
were
separated
fourths
sedimented
x g supernatant
freezing
in liquid
in
thawing
of the
and used as the 105,000
105,000
8 hours
from
the
5 and the preparation
three
was resuspended,
the
was
buffer
after
by
suspension
preparation,
When ribosomes
by aspiration
cell
30 minutes.
at -20'
2 hours.
x g pellet,
fraction.
x g for
and disrupted
pellet
The dialyzed
of activity.
removed
The 105,000
the ribosome
4 hours.
x g for
The broken
100 volumes
in small
in buffer
the resultant
at 30,000
i-t of Mg
at 105,000
was carefully
were
after
the concentration
psi.
30 minutes,
against
loss
suspended
at 16,000
Once thawed
and refreezing
g KCl,
centrifuged
was stored
nitrogen.
enzyme,
Press
x g for
fluid
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
and 0.06
a French
supernatant
natant
as,
BIOCHEMICAL
supernatant
x g super-
again
and used as
enzyme and ribosomes
nitrogen.
RESULTS AND DISCUSSION TablIe
I shows the requirements
The increase
is
dependent
and to a lesser degree
extent
of dependence
natent
is
shown here.
The increase inhibited REase ATCase is
II)..
by about
incorporation per
cent
OS a mixture inhibits
optimal
and the
14C labeled
of
cent.
widely
cent
amino
with
both
A)
The
different and a typical
the 105,000
of amino
respectively)
x g super-
of amino
acids
in activity
acids
of RNase which acids
into
are
by 5 ug of
the increase
incorporation
685
B).
to no effect
A concentration
14C labeled
(experiment
(experiment
incorporation
incorporation
L-leucine
in ATCase activity.
activity.
100 vg puromycin
even though 60 per
varies
C shows that
for
with
acids
dependency
(23 and 25 per
Flowever,
inhibited
acids
complete
in ATCase activity
is not
inhibited
amino
are required
to the same extent (Table
of amino
Experiment
increase
of ATP, GTP and Mg*
on the addition
from nearly
and ribosomes
an in vitro
on the addition
on exogenous
enzyme preparations experiment
for
protein
by more than
into
of
protein
inhibits by only
25
90 per
cent.
BIOCHEMICAL
Vol. 22, No. 6, 1966
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE I Requirements
for
an in vitro
increase
in ATCase activity milli-units
Experiment
A
Endogenous Complete 11 ,I
("enzyme"
I,
Experiment
buffer)
117 240
minus
ATP
125
GTP +I-
140 139
Mg
B
Endogenous Complete I,
plus
system II minus 11 minus
11 Experiment
ATCase
(~'enzyme" system 11
plus
122
buffer)
227 minus
amino
196
acids
C
Supernatant
enzyme plus
buffer
Supernatant
enzyme plus
incubation
Ribosomes
plus
buffer
Ribosomes
plus
incubation
135 mixture
172 18
mixture
42
Supernatant
plus
ribosomes
plus
buffer
Supernatant
plus
ribosomes
plus
incubation
,152 mixture
267
The complete system contained in pmoles: potassium phosphate 50 (pH 7.4); magnesium acetate 60; ATP 10; GTP 10; (all experimentally determined as being the optimal concentrations) phosphoenolpyruvate 5; 50 ngrams of each of the 20 amino acids and in experiments A and B about 1 mg of enzyme protein (Lowry et In experiment C 105,000 x g supernatant aZ., 1951) in a final volume of 1 ml. enzyme or ribosomes or the 105,000 x g supernatant plus ribosomes were incubated in buffer alone or in the complete reaction mixture. Incubation was for 10 minutes at 37O and the reaction was terminated by chilling the tubes in an ice From each tube 0.5 ml of the incubated reaction mixture was removed and bath. dialyzed for 3 hours against 100 volumes of O.OlM potassium phosphate buffer pH 7.4 containing 0.06 g KC1 with two changes of the buffer. The dialyzed incubation mixtures were then diluted to 5 ml with the above buffer and an aliquot assayed for ATCase by the method of Gerhart and Pardee (1962). One milli-unit of ATCase represents 1 mpmole of carbamylaspartate synthesized per minute under the conditions of the assay. Each experiment was repeated at least twice and assays run in duplicate. The duplicates rarely varied by more than 10 per cent.
686
Vol. 22, No. 6, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE II Effect
of RNase and puromycin
incorporation
of a mixture
of
on the in vitro 14C amino
increase ATCase
Complete
system
II
8,
II
II
acids
increase
of ATCase and on the
and 14C leucine
in
amino acids incorporated into protein
into
protein.
14C &-leucine incorporated into protein
milli-units
mm
56
57
43
42
3.3
56
22
3.5
plus 5 ug RNase
plus 100 ug puromycin
uumoles 56
Conditions as in Table I except that 5 pg of each of the 20 amino acids were used. For studies of the incorporation of labeled amino acids a mixture of 5 ug each of fifteen 14C amino acids ("Reconstituted protein hydrolysate" from Schwarz Bioresearch Inc., Orangeburg, N.Y.) and l'+C histidine were added to give 9.6 x lo5 cpm per tube. Five ug each of unlabeled aspargine, cysteine, For the studies of incorcystine, glutamine and methionine were also added. poration of labeled leucine, 5 pg of 14C Irleucine (specific activity 9 mc/tiJ and 5 pg each of the other 19 unlabeled aGino acids were added. In studies of inhibition of ATCase increase, 3 to 4 replicates were run as well as controls containing equivalent amounts of RNase or puromycin to rule out any possible inhibition of ATCase activity by these compounds. Control tubes for amino To measure the incorporaacids or leucine incorporation were incubated at O". tion of the label into protein the reaction was terminated by adding 5 ml of 5% trichloroacetate (TCA) and heated for 20 minutes at 90'. The precipitated protein was washed once with 5% TCA, then with 3:l ethanol:ether and then 5 times the filter containing the washed on a milliipore filter with 5% TCA. Finally precipitate was counted with 15 ml of scintillation fluid (10% napthalene, 0.7% 2,5-diphenyloxazole and 0.03% 2,2-p-phenylenebis(5-phenyloxazole) in reagent grade dioxane) in a liquid scintillgtion spectrometer. Endogenous values for ATCase and the control values (0 ) for the incorporation experiments have been subtracted. The conclentration amino that
acids
of puromycin
by about
inhibits inhibits
incorporation
cent
also
&-leucine
system
for
an in vitro
for
protein
of a mixture incorporation
of by more
90 per cent. The requirements
are
60 per
which
identical
of the
to the requirements
667
increase
synthesizing
in ATCase activity systems.
Therefore,
Vol. 22, No. 6, 1966
one is
inclined
ATCase.
to attribute
However,
hypothesis other
BIOCHEMICAL
is
not
processes.
conversion
the ohserved
results
obtained
entirely
adequate
The increase
heating
for
do
cause
1965)
puromycin
and a part
treatments
at 60'
an increase
with
of the
does not
known
or treatment
in our
to cause
with
synthesis
of
suggests
that
this
increase
must represent
seem to be due to the
form of the enzyme to its
since
4 minutes
to de nova
increase
in activity
of the oligomeric
and Schachman,
not
the
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
monomeric this
form
conversion,
ATP (Gerhart
(Gerhart such as
and Pardee,
1962),
system. ACKNOWLEDGEMENT
I wish
to thank
Professor
R. S. Bandurski
for
helpful
discussions.
REFERENCES Gerhart,
J.C.,
and Pardee,
Gerhart,
J.C.,
and Schachman,
Lowry, O.H., 193, 265,
Roseborough, (1951).
A.B.,
N.J.,
J.
H.K., Farr,
Nisman, B., and Pelmont, J., in J.N. in Nucleic Acid Research and Mol. 1964, p. 235.
Biol.
m.,
237,
Biochemistry, A.L.,
891,
(1962).
5, 1054,
(1965).
and Randall,
R.J.,
J.
Biol.
m.,
Davidson, and W.E. Cohn (Editors), Progress Biol., Academic Press Inc., New York,
688
AN IN
BIOCHEMICAL
lrITR0
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
INCREASE IN ASPARTYLTRANSCARBAMYLASE ACTIVITY* Raizada
MSU/AEC Plant
Received
Research
February
A number
tion
observed
with
have demonstrated
(cf.
Nisman
an increase
in a cell-free
When grown
of this
mutant
vitro
in ATCase activity
partially
Pathology
inhibited
of specific
is
cell-free
greater
by RNase, but
if
mutant
is
activity
of E. coli. about
and Schachman,
here
dependent
amino
12 per
cent
The in
1965).
on the presence
enzyme preparation
exogenous
communica-
(ATCase)
requiring
(Gerhart
enzymes
The following
ATCase contitutes
reported
+t and a dialyzed
in activity
1964).
from a uracil of uracil,
protein
The increase
and Pelmont,
amounts
of the soluble
of ATP, GTP and Mg
synthesis
of aspartyltranscarbamylase
system
on limiting
increase
and Plant
11, 1966
systems
deals
Singh
Laboratory and Department of Botany Michigan State University East Lansing, Michigan, 48823
of investigators
in cell-free
M.M.
of the mutant.
acids
are added
and is
not by puromycin. EXPERIMENTAL
The mutant containing all
limiting
subsequent
washed
was grown
aerobically
amounts
operations
in a standard
buffer
at 37'
of uracil performed
to early
log
phase
(8 pg/ml)'.
The cells
at 0 to 5'.
The harvested
containing
0.01 g potassium
in a medium
were cells
phosphateL
chilled
and
were pH 7.4,
*This investigation was supported in part by the U.S. Atomic Energy Commission, Contract No. AT(ll-l)-1338 and in part by research grant AM 05916 from the National Institutes of Health to Dr. R. S. Bandurski. 1 I thank Dr. .I. C. Gerhart for cating unpublished observations
providing regarding
the mutant of E. coZi and communisuitable growth conditions.
n
'Use of phosphate buffer during preparation tion medium more than doubled the increas.e observed with tris(hydroxymethyl)aminomethane
of the "enzymd'and in the incubain ATCase activity above that buffer at the same pH.
Vol. 22, No. 6, 1966
0.014
g magnesium
passage
through
centrifuged the
acetate
at 10,000
fluid
was dialyzed
a change
of buffer
with
"enzyme",
liquid
caused
centrifuged fluid natant.
stored
aliquots
the
Both
at -20'
after
of standard
enzyme was not
was raised
stored
to 0.03
About
quick
discarded,
and
The superfor
designated
quick
freezing
again
since
were
separated
fourths
sedimented
x g supernatant
freezing
in liquid
in
thawing
of the
and used as the 105,000
105,000
8 hours
from
the
5 and the preparation
three
was resuspended,
the
was
buffer
after
by
suspension
preparation,
When ribosomes
by aspiration
cell
30 minutes.
at -20'
2 hours.
x g pellet,
fraction.
x g for
and disrupted
pellet
The dialyzed
of activity.
removed
The 105,000
the ribosome
4 hours.
x g for
The broken
100 volumes
in small
in buffer
the resultant
at 30,000
i-t of Mg
at 105,000
was carefully
were
after
the concentration
psi.
30 minutes,
against
loss
suspended
at 16,000
Once thawed
and refreezing
g KCl,
centrifuged
was stored
nitrogen.
enzyme,
Press
x g for
fluid
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
and 0.06
a French
supernatant
natant
as,
BIOCHEMICAL
supernatant
x g super-
again
and used as
enzyme and ribosomes
nitrogen.
RESULTS AND DISCUSSION TablIe
I shows the requirements
The increase
is
dependent
and to a lesser degree
extent
of dependence
natent
is
shown here.
The increase inhibited REase ATCase is
II)..
by about
incorporation per
cent
OS a mixture inhibits
optimal
and the
14C labeled
of
cent.
widely
cent
amino
with
both
A)
The
different and a typical
the 105,000
of amino
respectively)
x g super-
of amino
acids
in activity
acids
of RNase which acids
into
are
by 5 ug of
the increase
incorporation
685
B).
to no effect
A concentration
14C labeled
(experiment
(experiment
incorporation
incorporation
L-leucine
in ATCase activity.
activity.
100 vg puromycin
even though 60 per
varies
C shows that
for
with
acids
dependency
(23 and 25 per
Flowever,
inhibited
acids
complete
in ATCase activity
is not
inhibited
amino
are required
to the same extent (Table
of amino
Experiment
increase
of ATP, GTP and Mg*
on the addition
from nearly
and ribosomes
an in vitro
on the addition
on exogenous
enzyme preparations experiment
for
protein
by more than
into
of
protein
inhibits by only
25
90 per
cent.
BIOCHEMICAL
Vol. 22, No. 6, 1966
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE I Requirements
for
an in vitro
increase
in ATCase activity milli-units
Experiment
A
Endogenous Complete 11 ,I
("enzyme"
I,
Experiment
buffer)
117 240
minus
ATP
125
GTP +I-
140 139
Mg
B
Endogenous Complete I,
plus
system II minus 11 minus
11 Experiment
ATCase
(~'enzyme" system 11
plus
122
buffer)
227 minus
amino
196
acids
C
Supernatant
enzyme plus
buffer
Supernatant
enzyme plus
incubation
Ribosomes
plus
buffer
Ribosomes
plus
incubation
135 mixture
172 18
mixture
42
Supernatant
plus
ribosomes
plus
buffer
Supernatant
plus
ribosomes
plus
incubation
,152 mixture
267
The complete system contained in pmoles: potassium phosphate 50 (pH 7.4); magnesium acetate 60; ATP 10; GTP 10; (all experimentally determined as being the optimal concentrations) phosphoenolpyruvate 5; 50 ngrams of each of the 20 amino acids and in experiments A and B about 1 mg of enzyme protein (Lowry et In experiment C 105,000 x g supernatant aZ., 1951) in a final volume of 1 ml. enzyme or ribosomes or the 105,000 x g supernatant plus ribosomes were incubated in buffer alone or in the complete reaction mixture. Incubation was for 10 minutes at 37O and the reaction was terminated by chilling the tubes in an ice From each tube 0.5 ml of the incubated reaction mixture was removed and bath. dialyzed for 3 hours against 100 volumes of O.OlM potassium phosphate buffer pH 7.4 containing 0.06 g KC1 with two changes of the buffer. The dialyzed incubation mixtures were then diluted to 5 ml with the above buffer and an aliquot assayed for ATCase by the method of Gerhart and Pardee (1962). One milli-unit of ATCase represents 1 mpmole of carbamylaspartate synthesized per minute under the conditions of the assay. Each experiment was repeated at least twice and assays run in duplicate. The duplicates rarely varied by more than 10 per cent.
686
Vol. 22, No. 6, 1966
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
TABLE II Effect
of RNase and puromycin
incorporation
of a mixture
of
on the in vitro 14C amino
increase ATCase
Complete
system
II
8,
II
II
acids
increase
of ATCase and on the
and 14C leucine
in
amino acids incorporated into protein
into
protein.
14C &-leucine incorporated into protein
milli-units
mm
56
57
43
42
3.3
56
22
3.5
plus 5 ug RNase
plus 100 ug puromycin
uumoles 56
Conditions as in Table I except that 5 pg of each of the 20 amino acids were used. For studies of the incorporation of labeled amino acids a mixture of 5 ug each of fifteen 14C amino acids ("Reconstituted protein hydrolysate" from Schwarz Bioresearch Inc., Orangeburg, N.Y.) and l'+C histidine were added to give 9.6 x lo5 cpm per tube. Five ug each of unlabeled aspargine, cysteine, For the studies of incorcystine, glutamine and methionine were also added. poration of labeled leucine, 5 pg of 14C Irleucine (specific activity 9 mc/tiJ and 5 pg each of the other 19 unlabeled aGino acids were added. In studies of inhibition of ATCase increase, 3 to 4 replicates were run as well as controls containing equivalent amounts of RNase or puromycin to rule out any possible inhibition of ATCase activity by these compounds. Control tubes for amino To measure the incorporaacids or leucine incorporation were incubated at O". tion of the label into protein the reaction was terminated by adding 5 ml of 5% trichloroacetate (TCA) and heated for 20 minutes at 90'. The precipitated protein was washed once with 5% TCA, then with 3:l ethanol:ether and then 5 times the filter containing the washed on a milliipore filter with 5% TCA. Finally precipitate was counted with 15 ml of scintillation fluid (10% napthalene, 0.7% 2,5-diphenyloxazole and 0.03% 2,2-p-phenylenebis(5-phenyloxazole) in reagent grade dioxane) in a liquid scintillgtion spectrometer. Endogenous values for ATCase and the control values (0 ) for the incorporation experiments have been subtracted. The conclentration amino that
acids
of puromycin
by about
inhibits inhibits
incorporation
cent
also
&-leucine
system
for
an in vitro
for
protein
of a mixture incorporation
of by more
90 per cent. The requirements
are
60 per
which
identical
of the
to the requirements
667
increase
synthesizing
in ATCase activity systems.
Therefore,
Vol. 22, No. 6, 1966
one is
inclined
ATCase.
to attribute
However,
hypothesis other
BIOCHEMICAL
is
not
processes.
conversion
the ohserved
results
obtained
entirely
adequate
The increase
heating
for
do
cause
1965)
puromycin
and a part
treatments
at 60'
an increase
with
of the
does not
known
or treatment
in our
to cause
with
synthesis
of
suggests
that
this
increase
must represent
seem to be due to the
form of the enzyme to its
since
4 minutes
to de nova
increase
in activity
of the oligomeric
and Schachman,
not
the
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
monomeric this
form
conversion,
ATP (Gerhart
(Gerhart such as
and Pardee,
1962),
system. ACKNOWLEDGEMENT
I wish
to thank
Professor
R. S. Bandurski
for
helpful
discussions.
REFERENCES Gerhart,
J.C.,
and Pardee,
Gerhart,
J.C.,
and Schachman,
Lowry, O.H., 193, 265,
Roseborough, (1951).
A.B.,
N.J.,
J.
H.K., Farr,
Nisman, B., and Pelmont, J., in J.N. in Nucleic Acid Research and Mol. 1964, p. 235.
Biol.
m.,
237,
Biochemistry, A.L.,
891,
(1962).
5, 1054,
(1965).
and Randall,
R.J.,
J.
Biol.
m.,
Davidson, and W.E. Cohn (Editors), Progress Biol., Academic Press Inc., New York,
688