BIOCHEMICAL
Vol.71,No.4,1976
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
GLUTATHIONE PEROXIDASE ACTIVITY IN SELENIUM-DEFICIENT Richard
A. Lawrence
Department of Internal Health Science Center Veterans Administration
Received
May 18,
RAT LIVER'
and Raymond F. Burk
Medicine, at Dallas Hospital,
University and Dallas,
of Texas Texas
75235
1976
SUMMARY: Glutathione peroxidase activity in the liver supernatant from rats me-deficient diet for 2 weeks was 8% of control when measured with H 0 but 42% of control when assayed with cumene hydroperoxide. Two peaks of g fZu athione peroxidase activity were present in the Sephadex G-150 gel filtration chromatogram of rat liver supernatant when 1.5 mM cumene hydroperoxide was used as substrate. Only the first peak was detected when 0.25 mM H 0 was used as substrate. The first peak was absent from chromatograms of Se- ii e f* 1cient rat liver supernatants; but the second peak, which eluted at a position corresponding to M.W. = 39,000, appeared unchanged. The second peak thus represents a second glutathione peroxidase activity which catalyzes the destruction of organic hydroperoxides but has little activity toward H202 and which persists in severe selenium deficiency. INTRODUCTION:
11.1.9) it
Glutathione
was discovered
(2).
This
sources
in various
intake
activity
most
investigators,
tion
of a variety
other
substrates
tial
glutathione
%upported (R.A.L.)
Se which
from
H202 (lo),
toward Since
glutathione
of organic such
grants
Copyright 0 I976 by Academic Press, Inc. All rights of reproduction in any form reserved.
tightly
bound
rat
the substrate
(ll),
952
form
from
(5,7,8)
liver
several
and its
on dietary
Se
has no glutathione
used for
its
assay
by
can catalyze
the
some workers
have used
With
has been reported
ROl ES-01017
and characterized
is dependent
Se-deficient
hydroperoxides
activity
purified
in homogeneous
peroxidase
EC 1.
H202 oxidoreductase,
species
as cumene hydroperoxide.
peroxidase
by U.S.P.H.S.
is
several
It has been shown that
(9).
peroxidase
been obtained
It contains tissues
(glutathione:
(1) who partially
by Mills
enzyme has since
(3,4,5,6).
activity
peroxidase
(R.F.B.)
this
substrate
destruc-
substan-
in Se-deficient
and T32 AM-07100
rat
BIOCHEMICAL
Vol. 71, No. 4, 1976
liver.
(12).
Using
dase activities
cumene hydroperoxide
that
were
14 months.
This
glutathione
peroxidase
finding
indicated which
activity
is
Se status,
a non-Se-dependent source
of error.
to resist
stress
from
activity,
which
fed
the
possible
not
be Se-dependent.
glutathione
studies
agents
should
not be measured rat
liver
the glutathione
peroxidase
Since
of the into
of the
for
glutathione or functional could
be an
ability
of an animal
account
such an
H202.
x 9 supernatants
activity
diet
of an additional
activity
with
peroxi-
a Se-deficient
nutritional
take
by assays
105,000
glutathione
existence
peroxidase
In addition,
oxidative
might
cumene hydroperoxide
in rats
used as a means of assessing
important
we have fractionated
might
RESEARCH COMMUNICATIONS
we have observed
30% of control
peroxidase
measured
AND BIOPHYSICAL
For these
on Sephadex fractions
reasons G-150
using
and
both
and H202 as substrates.
METHODS: Weanling male Holtzman rats were fed a Torula yeast-based Se-defimet (13) or the same diet supplemented with 0.5 mg Se as sodium selenite per Kg (controls). The rats were exsanguinated under ether anesthesia. The livers were perfused with 1.14 M NaCl and homogenized in 0.25 M sucrose. The supernatant fraction was prepared by centrifugation at 105,000 x 9 for 1 hour. Enzyme activity was measured by a modification of the coupled assay procedure of Paglia and Valentine (14). The reaction mixture consisted of 50 mM potassium phosphate buffer (pH 7), 1 mM EDTA, 1 mM NaN3, 0.2 mM NADPH, 1 E.U./ml GSSG-reductase, 1 mM GSH, 1.5 mM cumene hydroperoxlde or 0.25 mM H202 in a total volume of 1 ml. All ingredients except enzyme source and peroxide were combined at the beginning of each day. Enzyme source (0.1 ml) was added to 0.8 ml of the above mixture and allowed to incubate 5 min. at room temperature before initiation of the reaction by the addition of 0.1 ml peroxide solution. Absorbance at 340 nm was recorded for 5 min. and the activity was calculated from the slope of these lines as pmoles NADPH oxidized per minute. Blank reactions with enzyme source replaced by distilled water were subtracted from each assay. Protein was measured by the method of Lowry et al. (15). RESULTS AND DISCUSSION:
Table
liver
rats
supernatants
The activity
from
measured
with
1 shows glutathione fed Se-deficient
by 2 weeks
but
had decreased
much less,
to 42% of control.
Figure rats
fed
peroxidase
1 shows
the
gel
experimental
activity
and control
H202 had decreased
8% of control
the activity
filtration diets
appeared
in
3 months.
the chromatogram
953
in the
measured
chromatograms for
peroxidase
activity diets
Se-deficient
with
of liver Two peaks
in
for
2 weeks. rats
to
cumene hydroperoxide
supernatants
from
of glutathione
of the supernatant
from
the
Vol.71,No.4,
BIOCHEMICAL
1976
TABLE I: Effect on Rat Liver
AND BIOPHYSICALRESEARCH
of Dietary Glutathione
Selenium Supplementalion Peroxidase Activity
GSH-Peroxidase Dietary
COMMUNICATIONS
Activity*
f S.E.
Cumene.OOH
Se
0 wm
28 ?r 7.5
314 f 18
0.5
354 f 65
748 i 81
ppm
'Rats were fed the respective diets from weaning for 2 weeks before killing and processing as described in the text. 'Results are expressed min. per mg protein.
as pmoles NADPH oxidized per There were 4 rats per group.
A. CONTROL zo-
40
50
FRACTION
Fig.
1
Se-adequate the second cates
60
70
80
go-
NO. (-3mVFroctd
Sephadex G-150 gel filtration of rat liver supernatant. Gel filtration was performed on a 5 x 22.5 cm column of Sephadex G-150 eluted with 0.05 M tris buffer (pH 8.6) containing 1 n&l EDTA and 0.1 M .K2HPO4 at a flow rate of 60 ml/hr. The sample was applied in a 10 ml volume.
rat
(Fig.
1A) when cumene hydroperoxide
peak was not detected
the presence
of 2 glutathione
was used as substrate
when H202 was used as substrate. peroxidases
954
capable
of destroying
This
but indi-
cumene
BIOCHEMICAL
Vol.71,No.4,1976
hydroperoxid'e,
only
The chromatogram activity
but
1 of which
of the
AND BIOPHYSICAL
destroys
Se-deficient
Se-dependent
glutathione
peroxidase.
on the basis
of its
assay
conditions.
1B) showed
Peak I thus
Peak II
weight,
these (Fig.
II activity.
of peak
molecular
H202 under supernatant
persistence
RESEARCH COMMUNICATIONS
no peak I
appears
to be the
seems to be a different
substrate
specificity,
enzyme
and persistence
in Se deficiency. Our assay
procedure
measures
the oxidized
glutathione
peroxidase
reaction
by coupling
glutathione
reductase.
There
was a possibility,
catalyzed GSH.
the oxidation
We have also
of GSH remaining catalyzes Table
the
of NADPH directly
been able as described
oxidation
Time (min.)
it
to the oxidation therefore,
rather
to measure
this
by Hafeman,
formed
than
activity
et al.
in the of NADPH via
that
through
II
peak
oxidation
by direct
of
measurement
(10) indicating
that
peak
of GSH.
II shows results
TABLE II:
glutathione
Effect
of a heat
of Heating
denaturation
at 60' Peak I.
% of Control
experiment.
Peak II
C on GSH-Px Activity' Peak II % of Control
0
loo2
1002
10
50
0
20
20
0
30
10
0
'Aliquots of the combined fractions having peak I and peak II activity from Sephadex G-150 chromatography were heated in a thermostated water bath at 60" C. At the times indicated 0.1 ml samples were withdrawn, added to 0.8 ml ice cold reaction mixture, then allowed to incubate at room temperature for 5 minutes and assayed for GSH-Px activity as described in the text. 'Contained 0.2 enzyme units expressed as change in O.D. at 340 nm per minute for peak I and 0.38 enzyme units for peak II per ml.
955
II
BIOCHEMICAL
Vol. 71, No. 4, 1976
activity
is
I activity
is
provides the
completely still
further
protein
39,000
evidence
II
2.
after
of peak
peak II
of the
peak I enzyme,
at 60" C but
at 60"
This
C.
peak
at a volume G-150
peak
experiment
I and peak
by other
peroxidase
weight
II and of
has been found
II
enzyme could
.6r
I
as shown for
to contain
weight
I
column
the
(3,4,5,6).
about
be a dimer
I
to M.W. =
determined
investigators
enzyme has a molecular
the peak
corresponding superfine
the molecular
peroxidase
glutathione
and the
10 minutes
between
eluted
one-half
glutathione
(3,4,5,6)
30 minutes
on the Sephadex
is about
Se-dependent
for
II.
enzyme activity
This
Se-dependent
by heating
of a difference
when chromatographed
in Fig.
the
detectable
nature
The peak
destroyed
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Since 4 subunits
one-half
that
of the peak
I
1
K (1” .4 -
.3 -
I
4.2 Log
Fig.
2
H202.
that
retains
activity
M.W
no activity
in
does not dissociate
to give
peak
activity
toward
We have rechromatographed
and have observed
II
I
4.6
Molecular weight determination of glutathione peroxidase peak II. Rat liver supernatant was chromatographed on a 2.6 x 29.4 cm column of Sephadex G-150 superfine eluted with the same buffer as Fig. 1 at a flow rate of 6 mljhr. The sample was applied in a 1.5 ml volume. This column was calibrated using cytochrome c (M.W. = 12,384), achymotrypsin (M.W. = 22,500) and ovalbumin (W.W. = 45,000).
enzyme subunits toward
I
4.4
is
not diminished
peak
the peak II II
under
by severe
956
organic
hydroperoxides
I fractions region,
these
on Sephadex indicating
conditions.
Se deficiency,
but
it
that Also,
probably
not
G-150 peak since does
I peak
not
BIOCHEMICAL
Vol. 71, No. 4, 1976
contain
Se as does the
has not yet suggests turally
these
related,
would
differences
The onset
mentation
liver
diets
By increasing
II enzyme which
such
as the
sheep which
peak II
rat
which
trations
peroxidase
detected
I.
still
give
peroxidase at these
peak II
in
by Table should
glutathione
of the
separation
from
could
time
be struc-
of the
tissues
observed
(16).
substrate
where
both
using
results
indicate,
enzymes
of H202. so assay
peak
II
have much liver
the
present
assay
at the usual
G.C. G.C.
(1957) J. Biol. (1959) J. Biol. and FTbhq. 34B;l~;0-~52.and
::
%%$~h;m:
5.
J. Biol' Chem' 250 ch,m:,-%ithK'H.E.,
activity
specific must
for
51;4-ii49. and Hoeks tra,
957
W.G.
(1974)
the
be done after
m. 229, 189-197. Chem. z, 502-506. (1967 ) Hoppe-Seyler's Z. Sr ivastava, S.K. (1975)
l3-, 1825-1829.
concen-
cannot
REFERENCES: Mills, Mills,
of
as is
peak I enzyme.
::
in
activity.
enzyme activity
No substrate
of its
species
of peak I or Se-dependent
estimate the
this
in Se and
peak II for
are
H202 as substrate
since
for
in the
a problem
of
acids.
In addition,
than
low
by supple-
amino
necrosis
poses
diets
The existence
liver
I activity
peak
fed
can be delayed
I enzyme activity
peak
a reliable
activity,
in rats
provide
dietary
peak II enzyme
Assays
occurs
acids,
preliminary
has higher
concentrations
the
importance
in Se deficiencv.
develop
than
enzyme has been found
should
of the sulfur-containing they
may, as our
The existence
demonstrated
do not
they
or methionine
decreased
enzyme activity
to the
glutathione
effect
is not
E deficiency
contrast
which amino
the GSH concentration
peak
at this
them.
cysteine
this
the
II enzyme
peak
available
Even if
from
necrosis,
with
enzyme may explain
higher
detract
E and sulfur-containing
of these
vitamin
not
RESEARCH COMMUNICATIONS
of purified
The evidence enzymes.
between
of dietary
in Se, vitamin
Se analysis
however.
are 2 different
this
physiological
this
peak I enzyme.
been performed,
that
AND BIOPHYSICAL
Biochem.
be
Vol.71,No.4,
6.
7. 8. 9. 10.
11. 12. 13. 14.
1976
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Nakamura, W., Hosoda, S., and Hayashi , K. (1974) Biochem. Bio h s Acta 358, 251-261. !%$$$ m,Pope, A.L., Ganther, H .E., Swanson , A.B., Hafeand Hoekstra, W.G. (1973) Science 179-, 588-590. Flo;e,'L:: Gunzler, W.A., and Schock, H.H.973) FEBS Lett.
32. 132-134.
z&her, H.E., Hafeman, D.G., Lawrence, R.A., Serfass, R.E., and Hoekstra, W.G. (1976) in Trace Elements in Human Health and Disease (Prasad, A.S., Edmpress,cZemicPress,N.'f. HafemG., Sunde, R.A., and Hoekstra, W.G. (1974) J. Nutr. 104. 580-587. i?lGle, C., and O'Brien, P.J. (1968) Biochem. Biophys. Res. Commun. 31, 145-150. Chow, (:.c, and Tappel, A.L. (1974) J. Nutr. 104, 444-451. Burk, R.F., and Masters, B.S.S. (1975r -~ m. mchem. Biophys. l70, 124-131. Paglia, R.E., and Valentine, W.N. (1967) J- -Lab. -Clin. Med.
70, 158-169. 15. i&&y, O.H., Rosebrough, N.J., Farr, A.L., (1951) J. Biol. Chem. 193, 265-275. 16. Schwarz, K.v65)ed. &. 24, 58-67.
958
and Randall,
R.J.
Vol.71,No.4,1976
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
GLUTATHIONE PEROXIDASE ACTIVITY IN SELENIUM-DEFICIENT Richard
A. Lawrence
Department of Internal Health Science Center Veterans Administration
Received
May 18,
RAT LIVER'
and Raymond F. Burk
Medicine, at Dallas Hospital,
University and Dallas,
of Texas Texas
75235
1976
SUMMARY: Glutathione peroxidase activity in the liver supernatant from rats me-deficient diet for 2 weeks was 8% of control when measured with H 0 but 42% of control when assayed with cumene hydroperoxide. Two peaks of g fZu athione peroxidase activity were present in the Sephadex G-150 gel filtration chromatogram of rat liver supernatant when 1.5 mM cumene hydroperoxide was used as substrate. Only the first peak was detected when 0.25 mM H 0 was used as substrate. The first peak was absent from chromatograms of Se- ii e f* 1cient rat liver supernatants; but the second peak, which eluted at a position corresponding to M.W. = 39,000, appeared unchanged. The second peak thus represents a second glutathione peroxidase activity which catalyzes the destruction of organic hydroperoxides but has little activity toward H202 and which persists in severe selenium deficiency. INTRODUCTION:
11.1.9) it
Glutathione
was discovered
(2).
This
sources
in various
intake
activity
most
investigators,
tion
of a variety
other
substrates
tial
glutathione
%upported (R.A.L.)
Se which
from
H202 (lo),
toward Since
glutathione
of organic such
grants
Copyright 0 I976 by Academic Press, Inc. All rights of reproduction in any form reserved.
tightly
bound
rat
the substrate
(ll),
952
form
from
(5,7,8)
liver
several
and its
on dietary
Se
has no glutathione
used for
its
assay
by
can catalyze
the
some workers
have used
With
has been reported
ROl ES-01017
and characterized
is dependent
Se-deficient
hydroperoxides
activity
purified
in homogeneous
peroxidase
EC 1.
H202 oxidoreductase,
species
as cumene hydroperoxide.
peroxidase
by U.S.P.H.S.
is
several
It has been shown that
(9).
peroxidase
been obtained
It contains tissues
(glutathione:
(1) who partially
by Mills
enzyme has since
(3,4,5,6).
activity
peroxidase
(R.F.B.)
this
substrate
destruc-
substan-
in Se-deficient
and T32 AM-07100
rat
BIOCHEMICAL
Vol. 71, No. 4, 1976
liver.
(12).
Using
dase activities
cumene hydroperoxide
that
were
14 months.
This
glutathione
peroxidase
finding
indicated which
activity
is
Se status,
a non-Se-dependent source
of error.
to resist
stress
from
activity,
which
fed
the
possible
not
be Se-dependent.
glutathione
studies
agents
should
not be measured rat
liver
the glutathione
peroxidase
Since
of the into
of the
for
glutathione or functional could
be an
ability
of an animal
account
such an
H202.
x 9 supernatants
activity
diet
of an additional
activity
with
peroxi-
a Se-deficient
nutritional
take
by assays
105,000
glutathione
existence
peroxidase
In addition,
oxidative
might
cumene hydroperoxide
in rats
used as a means of assessing
important
we have fractionated
might
RESEARCH COMMUNICATIONS
we have observed
30% of control
peroxidase
measured
AND BIOPHYSICAL
For these
on Sephadex fractions
reasons G-150
using
and
both
and H202 as substrates.
METHODS: Weanling male Holtzman rats were fed a Torula yeast-based Se-defimet (13) or the same diet supplemented with 0.5 mg Se as sodium selenite per Kg (controls). The rats were exsanguinated under ether anesthesia. The livers were perfused with 1.14 M NaCl and homogenized in 0.25 M sucrose. The supernatant fraction was prepared by centrifugation at 105,000 x 9 for 1 hour. Enzyme activity was measured by a modification of the coupled assay procedure of Paglia and Valentine (14). The reaction mixture consisted of 50 mM potassium phosphate buffer (pH 7), 1 mM EDTA, 1 mM NaN3, 0.2 mM NADPH, 1 E.U./ml GSSG-reductase, 1 mM GSH, 1.5 mM cumene hydroperoxlde or 0.25 mM H202 in a total volume of 1 ml. All ingredients except enzyme source and peroxide were combined at the beginning of each day. Enzyme source (0.1 ml) was added to 0.8 ml of the above mixture and allowed to incubate 5 min. at room temperature before initiation of the reaction by the addition of 0.1 ml peroxide solution. Absorbance at 340 nm was recorded for 5 min. and the activity was calculated from the slope of these lines as pmoles NADPH oxidized per minute. Blank reactions with enzyme source replaced by distilled water were subtracted from each assay. Protein was measured by the method of Lowry et al. (15). RESULTS AND DISCUSSION:
Table
liver
rats
supernatants
The activity
from
measured
with
1 shows glutathione fed Se-deficient
by 2 weeks
but
had decreased
much less,
to 42% of control.
Figure rats
fed
peroxidase
1 shows
the
gel
experimental
activity
and control
H202 had decreased
8% of control
the activity
filtration diets
appeared
in
3 months.
the chromatogram
953
in the
measured
chromatograms for
peroxidase
activity diets
Se-deficient
with
of liver Two peaks
in
for
2 weeks. rats
to
cumene hydroperoxide
supernatants
from
of glutathione
of the supernatant
from
the
Vol.71,No.4,
BIOCHEMICAL
1976
TABLE I: Effect on Rat Liver
AND BIOPHYSICALRESEARCH
of Dietary Glutathione
Selenium Supplementalion Peroxidase Activity
GSH-Peroxidase Dietary
COMMUNICATIONS
Activity*
f S.E.
Cumene.OOH
Se
0 wm
28 ?r 7.5
314 f 18
0.5
354 f 65
748 i 81
ppm
'Rats were fed the respective diets from weaning for 2 weeks before killing and processing as described in the text. 'Results are expressed min. per mg protein.
as pmoles NADPH oxidized per There were 4 rats per group.
A. CONTROL zo-
40
50
FRACTION
Fig.
1
Se-adequate the second cates
60
70
80
go-
NO. (-3mVFroctd
Sephadex G-150 gel filtration of rat liver supernatant. Gel filtration was performed on a 5 x 22.5 cm column of Sephadex G-150 eluted with 0.05 M tris buffer (pH 8.6) containing 1 n&l EDTA and 0.1 M .K2HPO4 at a flow rate of 60 ml/hr. The sample was applied in a 10 ml volume.
rat
(Fig.
1A) when cumene hydroperoxide
peak was not detected
the presence
of 2 glutathione
was used as substrate
when H202 was used as substrate. peroxidases
954
capable
of destroying
This
but indi-
cumene
BIOCHEMICAL
Vol.71,No.4,1976
hydroperoxid'e,
only
The chromatogram activity
but
1 of which
of the
AND BIOPHYSICAL
destroys
Se-deficient
Se-dependent
glutathione
peroxidase.
on the basis
of its
assay
conditions.
1B) showed
Peak I thus
Peak II
weight,
these (Fig.
II activity.
of peak
molecular
H202 under supernatant
persistence
RESEARCH COMMUNICATIONS
no peak I
appears
to be the
seems to be a different
substrate
specificity,
enzyme
and persistence
in Se deficiency. Our assay
procedure
measures
the oxidized
glutathione
peroxidase
reaction
by coupling
glutathione
reductase.
There
was a possibility,
catalyzed GSH.
the oxidation
We have also
of GSH remaining catalyzes Table
the
of NADPH directly
been able as described
oxidation
Time (min.)
it
to the oxidation therefore,
rather
to measure
this
by Hafeman,
formed
than
activity
et al.
in the of NADPH via
that
through
II
peak
oxidation
by direct
of
measurement
(10) indicating
that
peak
of GSH.
II shows results
TABLE II:
glutathione
Effect
of a heat
of Heating
denaturation
at 60' Peak I.
% of Control
experiment.
Peak II
C on GSH-Px Activity' Peak II % of Control
0
loo2
1002
10
50
0
20
20
0
30
10
0
'Aliquots of the combined fractions having peak I and peak II activity from Sephadex G-150 chromatography were heated in a thermostated water bath at 60" C. At the times indicated 0.1 ml samples were withdrawn, added to 0.8 ml ice cold reaction mixture, then allowed to incubate at room temperature for 5 minutes and assayed for GSH-Px activity as described in the text. 'Contained 0.2 enzyme units expressed as change in O.D. at 340 nm per minute for peak I and 0.38 enzyme units for peak II per ml.
955
II
BIOCHEMICAL
Vol. 71, No. 4, 1976
activity
is
I activity
is
provides the
completely still
further
protein
39,000
evidence
II
2.
after
of peak
peak II
of the
peak I enzyme,
at 60" C but
at 60"
This
C.
peak
at a volume G-150
peak
experiment
I and peak
by other
peroxidase
weight
II and of
has been found
II
enzyme could
.6r
I
as shown for
to contain
weight
I
column
the
(3,4,5,6).
about
be a dimer
I
to M.W. =
determined
investigators
enzyme has a molecular
the peak
corresponding superfine
the molecular
peroxidase
glutathione
and the
10 minutes
between
eluted
one-half
glutathione
(3,4,5,6)
30 minutes
on the Sephadex
is about
Se-dependent
for
II.
enzyme activity
This
Se-dependent
by heating
of a difference
when chromatographed
in Fig.
the
detectable
nature
The peak
destroyed
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Since 4 subunits
one-half
that
of the peak
I
1
K (1” .4 -
.3 -
I
4.2 Log
Fig.
2
H202.
that
retains
activity
M.W
no activity
in
does not dissociate
to give
peak
activity
toward
We have rechromatographed
and have observed
II
I
4.6
Molecular weight determination of glutathione peroxidase peak II. Rat liver supernatant was chromatographed on a 2.6 x 29.4 cm column of Sephadex G-150 superfine eluted with the same buffer as Fig. 1 at a flow rate of 6 mljhr. The sample was applied in a 1.5 ml volume. This column was calibrated using cytochrome c (M.W. = 12,384), achymotrypsin (M.W. = 22,500) and ovalbumin (W.W. = 45,000).
enzyme subunits toward
I
4.4
is
not diminished
peak
the peak II II
under
by severe
956
organic
hydroperoxides
I fractions region,
these
on Sephadex indicating
conditions.
Se deficiency,
but
it
that Also,
probably
not
G-150 peak since does
I peak
not
BIOCHEMICAL
Vol. 71, No. 4, 1976
contain
Se as does the
has not yet suggests turally
these
related,
would
differences
The onset
mentation
liver
diets
By increasing
II enzyme which
such
as the
sheep which
peak II
rat
which
trations
peroxidase
detected
I.
still
give
peroxidase at these
peak II
in
by Table should
glutathione
of the
separation
from
could
time
be struc-
of the
tissues
observed
(16).
substrate
where
both
using
results
indicate,
enzymes
of H202. so assay
peak
II
have much liver
the
present
assay
at the usual
G.C. G.C.
(1957) J. Biol. (1959) J. Biol. and FTbhq. 34B;l~;0-~52.and
::
%%$~h;m:
5.
J. Biol' Chem' 250 ch,m:,-%ithK'H.E.,
activity
specific must
for
51;4-ii49. and Hoeks tra,
957
W.G.
(1974)
the
be done after
m. 229, 189-197. Chem. z, 502-506. (1967 ) Hoppe-Seyler's Z. Sr ivastava, S.K. (1975)
l3-, 1825-1829.
concen-
cannot
REFERENCES: Mills, Mills,
of
as is
peak I enzyme.
::
in
activity.
enzyme activity
No substrate
of its
species
of peak I or Se-dependent
estimate the
this
in Se and
peak II for
are
H202 as substrate
since
for
in the
a problem
of
acids.
In addition,
than
low
by supple-
amino
necrosis
poses
diets
The existence
liver
I activity
peak
fed
can be delayed
I enzyme activity
peak
a reliable
activity,
in rats
provide
dietary
peak II enzyme
Assays
occurs
acids,
preliminary
has higher
concentrations
the
importance
in Se deficiencv.
develop
than
enzyme has been found
should
of the sulfur-containing they
may, as our
The existence
demonstrated
do not
they
or methionine
decreased
enzyme activity
to the
glutathione
effect
is not
E deficiency
contrast
which amino
the GSH concentration
peak
at this
them.
cysteine
this
the
II enzyme
peak
available
Even if
from
necrosis,
with
enzyme may explain
higher
detract
E and sulfur-containing
of these
vitamin
not
RESEARCH COMMUNICATIONS
of purified
The evidence enzymes.
between
of dietary
in Se, vitamin
Se analysis
however.
are 2 different
this
physiological
this
peak I enzyme.
been performed,
that
AND BIOPHYSICAL
Biochem.
be
Vol.71,No.4,
6.
7. 8. 9. 10.
11. 12. 13. 14.
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z&her, H.E., Hafeman, D.G., Lawrence, R.A., Serfass, R.E., and Hoekstra, W.G. (1976) in Trace Elements in Human Health and Disease (Prasad, A.S., Edmpress,cZemicPress,N.'f. HafemG., Sunde, R.A., and Hoekstra, W.G. (1974) J. Nutr. 104. 580-587. i?lGle, C., and O'Brien, P.J. (1968) Biochem. Biophys. Res. Commun. 31, 145-150. Chow, (:.c, and Tappel, A.L. (1974) J. Nutr. 104, 444-451. Burk, R.F., and Masters, B.S.S. (1975r -~ m. mchem. Biophys. l70, 124-131. Paglia, R.E., and Valentine, W.N. (1967) J- -Lab. -Clin. Med.
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