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The mechanism of the diurnal variation of hepatic HMG-CoA reductase activity in the rat
BIOCHEMICAL
Vol. 45, No. 1, 1971
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
THF, MECHANISM OF THE DIURNAL VARIATION REDUCTASE ACTIVITY Malcolm Department
Received
Higgins,
Takashi
OF HEPATIC HMG-CoA
IN THE RAT
Kawachi*
and Harry
Rudney
of Biological Chemistry, University of Cincinnati College of Medicine, Cincinnati, Ohio 45219
July 26, 1971
SUMMARY. Direct measurements of the incorporation of 3H-leucine into highly purified 8-hydroxy-pmethylglutaryl CoA reductase (E.C. 1.1.1.34) have shown that the diurnal variation in activity observed in crude fractions is due to synthesis of new enzyme protein for approximately six hours, followed by complete cessation of synthesis for a duration of approximately 15 hours. The rate of degradation does not appear to be significantly altered. The molecular
mechanisms
mammals have been a recent
review
regulated
the
CoA reductase
drastically
reduced
by various
treatments
biliary
drainage
Lynen co,
(7),
and others
of the it
synthesis
of investigation
by several
laboratories
activity
as measured
after
cholesterol
feeding
such as Triton
WR 1339
Hamprecht
and Saucier
that
and/or
degradation
* Present
address
: National
MVA, mevalonic
large
Cancer acid;
(3),
2),
is
(6),
Research
HMG-CoA,
138
Institute,
or
N&isler
and
Dugan -et al -*
in the activity liver
due to changes inhibition
is
increased (4),
(8),
variations
enzyme while Center
and is
Hamprecht,
in mouse and rat is
fractions,
noradrenaline
and Rodwell
diurnal
phenomenon
of the
(for
of HMG-CoA to
in microsomal (e.g.,
Shapiro
synthesis this
reduction
and Lynen
(3),
in
of 8-hydroxy-P-methylglutaryl
enzyme,
Back,
of cholesterol
the NADPH dependent
have demonstrated
suggested
synthesis
of this
synthesis
Abbreviations: CoA.
of isoprenoid
by the
enzyme and cholesterol
has been
control
The hepatic
catalyzes
(5).
Kandutsch
1).
extent
which
The activity
MVA.
subject
see Ref.
to a major
of the
preparations; in the rate
of
by cholesterol Tokyo,
&hydroxy-P-methylglutaryl-
Japan.
BIOCHEMICAL
Vol. 45, No. 1, 1971
feeding
may be due to the action
AND BIOPHYSICAL
of an as yet
RESEARCH COMMUNICATIONS
undiscovered
inhibitor
(e.g.,
10). In the aforementioned redu.ctase
activity
to studying
the
synthesis
work
in crude
on the
preparation
was obtained
microsomal
regulation
is
of the isolated
incorporation
measurement
to determine
into
isolated
of HMG-CoA
A more direct the
enzyme protein.
of 3H-leucine
of HMG-CoA reductase
via
preparations.
of enzyme levels
and degradation
studies
data
the
rate
of
We report
highly
by Kawachi
approach
here
purified
and Rudney
(11).
Methods Assay
of HMG-CoA Reductase.
by Kawachi
and Rudney
of the reaction lactone,
with
dried
fraction,
after
applied
MVA-lactone (pH 7.0)
markers
was scraped The amount
hydroxamate
of Hinse Animals
obtained free
from
access
radioactive intraperitoneally.
layer
which
were
chloride
and Lupten
and Isolation
amino
acid
directly in the
and Grass1
Inc.,
other (12),
One
of nitrogen,
plate
benzene:acetone
gel (1:l
with
corresponding
v/v).
2 M NH2OH to MVA-
a scintillation
fraction
was
of silica
successively
into
Female Madison,
chow and water.
dissolved
After
two aliquots.
The ether
counter
was determined
by the
or by the gas chromatographic
(13).
Sprague-Dawley, rat
into
The area
solution.
of Enzyme.
to Rockland
(5 x 1 vol).
with
of MVAwith
ether
chromatographic
termination
quantity
solution
by a stream
by spraying
the plate
of Lynen
volume
was developed
visualized
from
diethyl
as described After
known of the
was divided
to a small
of MVA-lactone
method
of an accurately
Na2SO4,
thickness),
were
1 ml or 2 ml volumes.
with
to a thin
and a ferric
lactone
method
was extracted
evaporation
mm wet
using
conditions
H2SO4 and saturation
by anhydrous
quantitatively
vial.
with
MYA-lactone
extract,
but
NaOH, addition
acidification
Na2SO4,
G (0.3
(11)
Incubation
in
rats,
Wisconsin, At
the
0.1 ml isotonic
an appropriate
139
time
approx
interval
200 g, were
and were specified saline
allowed
times
the
was injected
the rats
were
killed
BIOCHEMICAL
Vol. 45, No. 1, 1971
by decapitation, isotonic
or injected
AND BIOPHYSICAL
with
RESEARCH COMMUNICATIONS
25 mg unlabelled
leucine
dissolved
in
saline.
HMG-CoA reductase Kawachi
and Rudney
material
was isolated
(11)
through
was contaminated
accordkg
to the method
chromatography
by a minor
on Sephadex
component
(as shown
described G-200.
by This
by disc
gel
electrophoresis). Results Table from
the
specific tion
livers
the data
of rats
from
injected
radioactivity
stepis
of the Table
1 displays
and Discussion
with
and specific
evidence
that
an HMG-CoA reductase 3H-leucine. enzyme
purified
The correspondence
activity
the radioactivity
preparation
observed
in the is
final
indeed
in
purificaconstitutive
enzyme molecule. 1.
Purification
of 31NiMG-CoA-Reductase
Enzyme Activity
from Rat Liver
mg Protein
% Recovery of Activity
3H dpm
dpm 3H/mg Protein
Microsomal fraction
1.9
890
100
1.35
x 106
1,521
Deoxycholate supernatant
5.7
425
140
6.05
x
1,400
Ammonium sulfate fraction
10.1
169
109
2.48
x lo5
1,470
DEAR cellulose
78.0
18.1
82
3.5 x 104
1,950
Hydroxyapatite
277.0
3.1
51
7.65
x lo3
2,470
G-200
301
2.7
49
7.0 x 103
2,630
-
0.5
w
1.35
2,700
Sephadex
Disc -gel electrophoresis
*
lo5
x 103
Twenty rats were injected Fntraperitoneally with 50 p.Cf each of 3H-leucine (390 uCi/nmtole) in 0.1 ml isotonic saline. Protein in column fractions was precipitated with trichloroacetic acid after addition of 1 mg bovine albumen to each tube and filtered on Whatman 3GA discs. After digestion with Beckman Soluene-100 radioactivity was determined directly using a toluene based scintillant. Protein was determined by the Lowry-Folin methot. Enzyme activities expressed as nmoles MVA/mg protein/hr. 0.5 mg protein was subjected to polyacrylamide disc gel electrophoresis in 12 tubes. Gels were sliced, dissolved in piperidine and counted (15).
140
Vol. 45, No. 1, 1971
BIOCHEMICAL
Figure
obtained
1 shows data
the injection at each the
with
time
3H-leucine.
poFnt
same rats,
and the
AND BIOPHYSICAL
by isolation
of the
The microsomal
enzymic
total
radioactivity
was subsequently
RESEARCH COMMUNICATIONS
enzyme 35 min after activity
was measured
of the purified
enzyme,
from
determined.
. 280 240 200 160 120
0800
I200
1600
TIME
2000
2400
“; k$. Q +! s zi k
0400
OF DAY
Figure 1. Variation of Microsomal HMG-CoA Reductase Activity and Incorporatjon of 3H-leucine. Groups of 8 rats were injected with 40 p,Ci of H-leucine (390 mCi/mmole) at the times shown. Livers were removed 35 min later and enzyme purification commenced. Assays are a8 described in the text and legend to Table 1.
The specific the diurnal reflect8
activity
variation the rise
the diurnal remains
period;
constant
for could
indicate
and fall
of the
however,
an artifact
synthesie
purified
enzymes
The variation
the It
seems to precede
may be merely increased
period.
as expected.
in incorporation This
of the
is the
of the
of protein
a more complex
control
in crude
radioactivity interesting rise
of leucine fractions
that
in microsomal
during fractions
the
enzymic
reflecting
to be reflected
during
in microsomal to note
system,
where
change
in incorporation
enzyme activity total
does not
increase activity.
the time
required
a8 enzyme activity,
the enzyme
is
inhibited
or it at that
time. .A88uming
that
the
incorporation
of amino
141
acid
reflects
enzymic
syn-
BIOCHEMICAL
Vol. 45, No. 1, 1971
thesis
(and
since
not
decrease
begin
to feed
diurnal
variation
the animals
suggest
that
change
in rate
the
degradation then
of synthesis.
of the
35 min later
and specific time
tion In the
before
former
rapidly,
case,
while
Conversely,
in Figure
total
specific
of rats
time
is
were
diluted
into
the role with
were
and the
of these after by newly
played
determined
and the
essentially
is
results approximately synthesized
labeled is
at
fnjec-
striking. declines
constant,
of isolatable
“pulse”
by
3H-leucine,
and protein
amount
of the
due to a
the results
to increase
remains
to
radioactivity
between
radioactivity
radioactivity
not
partly
of maximum incorporation
isolatable
stops
least
The total
starts
here
was reasonable
injected
The contrast
radioactivity
essentially
is at
- unlikely
?lMG-CoA reductase
time
activity
it
leucine.
2.
Our explanation
rapidly.
size
some insight
of incorporation
the enzyme
the
at this
rate
specific
new enzyme protein labeled
groups
at the
the
the
while
rising,
decreased
the
pool
in enzyme
of purified
injections
acid
RESEARCH COMMUNICATIONS
at the same time),
25 mg unlabeled
as shown
from
just
protein, with
in amino
To gain
radioactivity
intervals
obtained
were
a large
AND BIOPHYSICAL
that six
protein protein
synthesis hours.
of Rrotein
enzyme.
*9* \P
DECREASING ENZYMIC ACTIVITI
t
2 14 :: 1 IO 2 $6 B $2 z sG
I2345678
12345678
TIME (in hours 1 Figure 2. The Variation of Specific Radioactivity after a Single Injection of 3H- leucine . Groups of 36 rats ware injected with 25 @i 3H-leucine each (440 l.UX/mmole) at 2200 hr (A) or 1630 hr (B) and with 25 mg unlabeled leucine 35 min later. Livers of 6 rats were excised at the times shown and the enzyme isolated. Rotted lines represent specific radioactivity, histogram the total radioactivity.
142
Vol. 45, No. 1, 1971
BIOCHEMICAL
The isolatable is plotted
radi.oactivity
on semilogarithmic
both while the enzyme activity while it is falling, data the half differences the
life
AND BIOPHYSICAL
at intervals
scales (Fig. 3).
after
RESEARCH COMMUNICATIONS
a single pulse label
The decay in radioactivity,
in the q icrosomal fraction
follows approximately of the protein
first
is rising
order kinetics.
is approximately
3 hr.
and From this
The slight
in slope of the two lines can be explained by reutilization
of
radioact ive amino acid.
TIME
(hours)
Associated with RMC-CoAReductase. Figure 3. Decay of Radioactivity Experimental conditions are as described for Figure 2. If
the assumption is made that the enzyme behaves identically
purification
procedures at high and low levels,
experiments (which will inhibitor equivocally
and in the light
be reported elsewhere) which failed
of the enzyme during the low part of the cycle, demonstrates that the diurnal variation
in the of mixing
to show an this data un-
in activity
is due to
an increase in the rate of synthesis of the enzyme during the rising
portion
of the cycle and an apparent complete cessation of enzyme synthesis during the
falling
phase. Present experimental conditions make it difficult
pin point the exact initiation
of these 143
to
phases. Changes in the rate of
BIOCHEMICAL
Vol. 45, No. 1, 1971
degradation
do not
AND BIOPHYSICAL
seem to be significantly
RESEARCH COMMUNICATIONS
different
during
both
phases .
of
the cycle. The conclusion rather
than
data
a marked
obtained
Randutsch using
that
it
change
by others
and Saucier
puromycin,
prevention
of the decrease
protein
also
with
a very
sis
playing
a role
the
signals
for
work
on complete
variation
* 9 * P \
is
was supported
Diseases,
Grant
Foundation
in activity
on the
by cycloheximide is
effected
repression
by a
The nature of the
of
synthesis
to be investigated.
by the National
No. AM-12402.
(14)
of enzyme synthe-
of note.
remains
work
synthesis.
any light
derepression
biosynthesis
rise
with
in the experiments
throw
worthy
and subsequent
the Wellcome
cyclic
about
of thia
This
from
brought
life.
and Metabolic grant
do not
half
Acknowledgements.
a travel
the
short
the repression
of protein
of RMG-CoA reductase
key enzyme in isoprenoid
of Arthritis
to prevent
in activity
in a diurnal
is consistent
inhibitors
Our results
(14).
of enzyme synthesis,
had the same effect
the degradation
The demonstration
of this
able
rate
of degradation,
antibiotic
cycloheximide
and Rodwell
changing
in the rate
using
of Shapiro
of course,
a rapidly
(3) were
while
unless,
is
Institute
MR acknowledges
(London).
DECREASING ENZYMlC *CT,“,Ty
t 2 14 :: 1 IO 2 $6 B $2 z G s
I2345678
12345678
TIME (in hours 1
Figure 2. The Variation of Specific Radioactivity after a Single Injection of 3H- leucine . Groups of 36 rats ware injected with 25 @i 3H-leucine each (440 uCi/mmole) at 2200 hr (A) or 1630 hr (B) and with 25 mg unlabeled leucine 35 min later. Livers of 6 rats were excised at the times shown and the enzyme isolated. Dotted lines represent specific radioactivity, histogram the total radioactivity.
142
Vol. 45, No. 1, 1971
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
THF, MECHANISM OF THE DIURNAL VARIATION REDUCTASE ACTIVITY Malcolm Department
Received
Higgins,
Takashi
OF HEPATIC HMG-CoA
IN THE RAT
Kawachi*
and Harry
Rudney
of Biological Chemistry, University of Cincinnati College of Medicine, Cincinnati, Ohio 45219
July 26, 1971
SUMMARY. Direct measurements of the incorporation of 3H-leucine into highly purified 8-hydroxy-pmethylglutaryl CoA reductase (E.C. 1.1.1.34) have shown that the diurnal variation in activity observed in crude fractions is due to synthesis of new enzyme protein for approximately six hours, followed by complete cessation of synthesis for a duration of approximately 15 hours. The rate of degradation does not appear to be significantly altered. The molecular
mechanisms
mammals have been a recent
review
regulated
the
CoA reductase
drastically
reduced
by various
treatments
biliary
drainage
Lynen co,
(7),
and others
of the it
synthesis
of investigation
by several
laboratories
activity
as measured
after
cholesterol
feeding
such as Triton
WR 1339
Hamprecht
and Saucier
that
and/or
degradation
* Present
address
: National
MVA, mevalonic
large
Cancer acid;
(3),
2),
is
(6),
Research
HMG-CoA,
138
Institute,
or
N&isler
and
Dugan -et al -*
in the activity liver
due to changes inhibition
is
increased (4),
(8),
variations
enzyme while Center
and is
Hamprecht,
in mouse and rat is
fractions,
noradrenaline
and Rodwell
diurnal
phenomenon
of the
(for
of HMG-CoA to
in microsomal (e.g.,
Shapiro
synthesis this
reduction
and Lynen
(3),
in
of 8-hydroxy-P-methylglutaryl
enzyme,
Back,
of cholesterol
the NADPH dependent
have demonstrated
suggested
synthesis
of this
synthesis
Abbreviations: CoA.
of isoprenoid
by the
enzyme and cholesterol
has been
control
The hepatic
catalyzes
(5).
Kandutsch
1).
extent
which
The activity
MVA.
subject
see Ref.
to a major
of the
preparations; in the rate
of
by cholesterol Tokyo,
&hydroxy-P-methylglutaryl-
Japan.
BIOCHEMICAL
Vol. 45, No. 1, 1971
feeding
may be due to the action
AND BIOPHYSICAL
of an as yet
RESEARCH COMMUNICATIONS
undiscovered
inhibitor
(e.g.,
10). In the aforementioned redu.ctase
activity
to studying
the
synthesis
work
in crude
on the
preparation
was obtained
microsomal
regulation
is
of the isolated
incorporation
measurement
to determine
into
isolated
of HMG-CoA
A more direct the
enzyme protein.
of 3H-leucine
of HMG-CoA reductase
via
preparations.
of enzyme levels
and degradation
studies
data
the
rate
of
We report
highly
by Kawachi
approach
here
purified
and Rudney
(11).
Methods Assay
of HMG-CoA Reductase.
by Kawachi
and Rudney
of the reaction lactone,
with
dried
fraction,
after
applied
MVA-lactone (pH 7.0)
markers
was scraped The amount
hydroxamate
of Hinse Animals
obtained free
from
access
radioactive intraperitoneally.
layer
which
were
chloride
and Lupten
and Isolation
amino
acid
directly in the
and Grass1
Inc.,
other (12),
One
of nitrogen,
plate
benzene:acetone
gel (1:l
with
corresponding
v/v).
2 M NH2OH to MVA-
a scintillation
fraction
was
of silica
successively
into
Female Madison,
chow and water.
dissolved
After
two aliquots.
The ether
counter
was determined
by the
or by the gas chromatographic
(13).
Sprague-Dawley, rat
into
The area
solution.
of Enzyme.
to Rockland
(5 x 1 vol).
with
of MVAwith
ether
chromatographic
termination
quantity
solution
by a stream
by spraying
the plate
of Lynen
volume
was developed
visualized
from
diethyl
as described After
known of the
was divided
to a small
of MVA-lactone
method
of an accurately
Na2SO4,
thickness),
were
1 ml or 2 ml volumes.
with
to a thin
and a ferric
lactone
method
was extracted
evaporation
mm wet
using
conditions
H2SO4 and saturation
by anhydrous
quantitatively
vial.
with
MYA-lactone
extract,
but
NaOH, addition
acidification
Na2SO4,
G (0.3
(11)
Incubation
in
rats,
Wisconsin, At
the
0.1 ml isotonic
an appropriate
139
time
approx
interval
200 g, were
and were specified saline
allowed
times
the
was injected
the rats
were
killed
BIOCHEMICAL
Vol. 45, No. 1, 1971
by decapitation, isotonic
or injected
AND BIOPHYSICAL
with
RESEARCH COMMUNICATIONS
25 mg unlabelled
leucine
dissolved
in
saline.
HMG-CoA reductase Kawachi
and Rudney
material
was isolated
(11)
through
was contaminated
accordkg
to the method
chromatography
by a minor
on Sephadex
component
(as shown
described G-200.
by This
by disc
gel
electrophoresis). Results Table from
the
specific tion
livers
the data
of rats
from
injected
radioactivity
stepis
of the Table
1 displays
and Discussion
with
and specific
evidence
that
an HMG-CoA reductase 3H-leucine. enzyme
purified
The correspondence
activity
the radioactivity
preparation
observed
in the is
final
indeed
in
purificaconstitutive
enzyme molecule. 1.
Purification
of 31NiMG-CoA-Reductase
Enzyme Activity
from Rat Liver
mg Protein
% Recovery of Activity
3H dpm
dpm 3H/mg Protein
Microsomal fraction
1.9
890
100
1.35
x 106
1,521
Deoxycholate supernatant
5.7
425
140
6.05
x
1,400
Ammonium sulfate fraction
10.1
169
109
2.48
x lo5
1,470
DEAR cellulose
78.0
18.1
82
3.5 x 104
1,950
Hydroxyapatite
277.0
3.1
51
7.65
x lo3
2,470
G-200
301
2.7
49
7.0 x 103
2,630
-
0.5
w
1.35
2,700
Sephadex
Disc -gel electrophoresis
*
lo5
x 103
Twenty rats were injected Fntraperitoneally with 50 p.Cf each of 3H-leucine (390 uCi/nmtole) in 0.1 ml isotonic saline. Protein in column fractions was precipitated with trichloroacetic acid after addition of 1 mg bovine albumen to each tube and filtered on Whatman 3GA discs. After digestion with Beckman Soluene-100 radioactivity was determined directly using a toluene based scintillant. Protein was determined by the Lowry-Folin methot. Enzyme activities expressed as nmoles MVA/mg protein/hr. 0.5 mg protein was subjected to polyacrylamide disc gel electrophoresis in 12 tubes. Gels were sliced, dissolved in piperidine and counted (15).
140
Vol. 45, No. 1, 1971
BIOCHEMICAL
Figure
obtained
1 shows data
the injection at each the
with
time
3H-leucine.
poFnt
same rats,
and the
AND BIOPHYSICAL
by isolation
of the
The microsomal
enzymic
total
radioactivity
was subsequently
RESEARCH COMMUNICATIONS
enzyme 35 min after activity
was measured
of the purified
enzyme,
from
determined.
. 280 240 200 160 120
0800
I200
1600
TIME
2000
2400
“; k$. Q +! s zi k
0400
OF DAY
Figure 1. Variation of Microsomal HMG-CoA Reductase Activity and Incorporatjon of 3H-leucine. Groups of 8 rats were injected with 40 p,Ci of H-leucine (390 mCi/mmole) at the times shown. Livers were removed 35 min later and enzyme purification commenced. Assays are a8 described in the text and legend to Table 1.
The specific the diurnal reflect8
activity
variation the rise
the diurnal remains
period;
constant
for could
indicate
and fall
of the
however,
an artifact
synthesie
purified
enzymes
The variation
the It
seems to precede
may be merely increased
period.
as expected.
in incorporation This
of the
is the
of the
of protein
a more complex
control
in crude
radioactivity interesting rise
of leucine fractions
that
in microsomal
during fractions
the
enzymic
reflecting
to be reflected
during
in microsomal to note
system,
where
change
in incorporation
enzyme activity total
does not
increase activity.
the time
required
a8 enzyme activity,
the enzyme
is
inhibited
or it at that
time. .A88uming
that
the
incorporation
of amino
141
acid
reflects
enzymic
syn-
BIOCHEMICAL
Vol. 45, No. 1, 1971
thesis
(and
since
not
decrease
begin
to feed
diurnal
variation
the animals
suggest
that
change
in rate
the
degradation then
of synthesis.
of the
35 min later
and specific time
tion In the
before
former
rapidly,
case,
while
Conversely,
in Figure
total
specific
of rats
time
is
were
diluted
into
the role with
were
and the
of these after by newly
played
determined
and the
essentially
is
results approximately synthesized
labeled is
at
fnjec-
striking. declines
constant,
of isolatable
“pulse”
by
3H-leucine,
and protein
amount
of the
due to a
the results
to increase
remains
to
radioactivity
between
radioactivity
radioactivity
not
partly
of maximum incorporation
isolatable
stops
least
The total
starts
here
was reasonable
injected
The contrast
radioactivity
essentially
is at
- unlikely
?lMG-CoA reductase
time
activity
it
leucine.
2.
Our explanation
rapidly.
size
some insight
of incorporation
the enzyme
the
at this
rate
specific
new enzyme protein labeled
groups
at the
the
the
while
rising,
decreased
the
pool
in enzyme
of purified
injections
acid
RESEARCH COMMUNICATIONS
at the same time),
25 mg unlabeled
as shown
from
just
protein, with
in amino
To gain
radioactivity
intervals
obtained
were
a large
AND BIOPHYSICAL
that six
protein protein
synthesis hours.
of Rrotein
enzyme.
*9* \P
DECREASING ENZYMIC ACTIVITI
t
2 14 :: 1 IO 2 $6 B $2 z sG
I2345678
12345678
TIME (in hours 1 Figure 2. The Variation of Specific Radioactivity after a Single Injection of 3H- leucine . Groups of 36 rats ware injected with 25 @i 3H-leucine each (440 l.UX/mmole) at 2200 hr (A) or 1630 hr (B) and with 25 mg unlabeled leucine 35 min later. Livers of 6 rats were excised at the times shown and the enzyme isolated. Rotted lines represent specific radioactivity, histogram the total radioactivity.
142
Vol. 45, No. 1, 1971
BIOCHEMICAL
The isolatable is plotted
radi.oactivity
on semilogarithmic
both while the enzyme activity while it is falling, data the half differences the
life
AND BIOPHYSICAL
at intervals
scales (Fig. 3).
after
RESEARCH COMMUNICATIONS
a single pulse label
The decay in radioactivity,
in the q icrosomal fraction
follows approximately of the protein
first
is rising
order kinetics.
is approximately
3 hr.
and From this
The slight
in slope of the two lines can be explained by reutilization
of
radioact ive amino acid.
TIME
(hours)
Associated with RMC-CoAReductase. Figure 3. Decay of Radioactivity Experimental conditions are as described for Figure 2. If
the assumption is made that the enzyme behaves identically
purification
procedures at high and low levels,
experiments (which will inhibitor equivocally
and in the light
be reported elsewhere) which failed
of the enzyme during the low part of the cycle, demonstrates that the diurnal variation
in the of mixing
to show an this data un-
in activity
is due to
an increase in the rate of synthesis of the enzyme during the rising
portion
of the cycle and an apparent complete cessation of enzyme synthesis during the
falling
phase. Present experimental conditions make it difficult
pin point the exact initiation
of these 143
to
phases. Changes in the rate of
BIOCHEMICAL
Vol. 45, No. 1, 1971
degradation
do not
AND BIOPHYSICAL
seem to be significantly
RESEARCH COMMUNICATIONS
different
during
both
phases .
of
the cycle. The conclusion rather
than
data
a marked
obtained
Randutsch using
that
it
change
by others
and Saucier
puromycin,
prevention
of the decrease
protein
also
with
a very
sis
playing
a role
the
signals
for
work
on complete
variation
* 9 * P \
is
was supported
Diseases,
Grant
Foundation
in activity
on the
by cycloheximide is
effected
repression
by a
The nature of the
of
synthesis
to be investigated.
by the National
No. AM-12402.
(14)
of enzyme synthe-
of note.
remains
work
synthesis.
any light
derepression
biosynthesis
rise
with
in the experiments
throw
worthy
and subsequent
the Wellcome
cyclic
about
of thia
This
from
brought
life.
and Metabolic grant
do not
half
Acknowledgements.
a travel
the
short
the repression
of protein
of RMG-CoA reductase
key enzyme in isoprenoid
of Arthritis
to prevent
in activity
in a diurnal
is consistent
inhibitors
Our results
(14).
of enzyme synthesis,
had the same effect
the degradation
The demonstration
of this
able
rate
of degradation,
antibiotic
cycloheximide
and Rodwell
changing
in the rate
using
of Shapiro
of course,
a rapidly
(3) were
while
unless,
is
Institute
MR acknowledges
(London).
DECREASING ENZYMlC *CT,“,Ty
t 2 14 :: 1 IO 2 $6 B $2 z G s
I2345678
12345678
TIME (in hours 1
Figure 2. The Variation of Specific Radioactivity after a Single Injection of 3H- leucine . Groups of 36 rats ware injected with 25 @i 3H-leucine each (440 uCi/mmole) at 2200 hr (A) or 1630 hr (B) and with 25 mg unlabeled leucine 35 min later. Livers of 6 rats were excised at the times shown and the enzyme isolated. Dotted lines represent specific radioactivity, histogram the total radioactivity.
142