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Invitro formation of assimilatory nitrate reductase: Presence of the constitutive component in bacteria
BIOCHEMICAL
Vol. 52, No. 4, 1973
--In Vitro
Formation
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of Assimilatory
of the Constitutive
Nitrate Component
Reductase:
Presence
in Bacteria.
Paul A. Ketchum and Ruth S. Swarin Department of Biological Sciences Oakland University Rochester, Michigan 48063
Received
April
23,
1973 ABSTRACT
Cell-free extracts of a selected group of bacteria which are capable of metabolyzing dinitrogen and/or nitrate contain a soluble form of the constitutive component which is active in the --in vitro formation of NADPH-nitrate reductase when mixed with extracts of N. crassa The constitutive component in these extracts is-dialyzabie --nit-l. and is insensitive to trypsin and protease. The constitutive component which substitutes for the absence of the --nit-l gene product in the --in vitro formation of NADPH-nitrate reductase is postulated to be a low molecular weight cofactor or polypeptide and is shown to be present in a number of unrelated bacteria. INTRODUCTION The Neurospora
assimilatory
oxidoreductase,
E.C.1.6.6.2.)
heteromultimeric
protein,
chrome 557 fied
(l-6).
evidence
flavin suggests
of NADPH-nitrate the
flavin
(9),
have
by mixing contains wild
type
at least
reductase
stimulated
the
four
in -*N
crassa,
The component
contributed
from
associated
with
-N. -3crassa
mutants
of 2.
uninduced
reductase
in the
one of which (7,8).
of NADPH-nitrate
-c reductase,
the
involved
at least
reductase which
with
extracts
extracts
other
and
Genetic formation codes
for
Nason et al.,
nit-l --2
crassa
puri-
NADPH-(FAD)-cyto-
reductase.
c reductase
induced
reductase
and cyto-
(MVH) nitrate
are
dalton,
molybdenum
reductase,
genes
formation
of nitrate
230,000
(FADH2) nitrate
the NADPH-(FAD)-cytochrome or nitrate
are
viologen
NADPH-cytochrome
demonstrated
flavin,
activities
dinucleotide
that
extracts
contains
methyl
(NADPH-nitrate:
inducible
NADPH-nitrate
reduced
adenine
reductase
a nitrate
enzymatic
reductase:
chrome -c reductase, reduced
is which
Four
NADPH-nitrate
NADPII-nitrate
--in vitro specifically of uninduced
than -nit-l --
to the --in vitro
BIOCHEMICAL
Vol. 52, No. 4, 1973
formation
of NADPH-nitrate
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
reductase
is
called
the
constitutive
compon-
ent. Pateman
et al.,
"common
cofactor"
in Aspergillus
nidulans
nitrate
reductase
and xanthine
dehydrogenase
(11)
(10)
demonstrated
that
enzymes
xanthine
tribute
the
nitrate
reductase
oxidase,
nitrate
enzymes
with
the
constitutive
Nason et al.,
(11,12). that
Acid
the
oxidase,
formation
have been
In explaining
can also of NADPH-
containing
shown
these
constitutive
treated
reductase
the known molybdenum
component
nitrate,
similar the
sensitive
to the --in vitro
con-
of NADPH-
sulfite
nitrate
(13)
oxidase
formation treated.
both
containing
and aldehyde
acid
a
et al.,
of the molybdenum
respiratory
all
for
Ketchum
nitrogenase),
of hydrogenase
demonstrates
can reduce
that
Therefore
is
necessary
activity.
first
(from
component
postulated
is
there
to contain
observations,
component
is
a moly-
cofactor.
pap'er
ments
are
exception
(12)
which
that
to the --in vitro
and --E. coli
(12).
evidence
dehydrogenase
enzymes
the constitutive reductase
This
these
reductase
nitrate
bdenum
xanthine component
if
genetic
preparations
of the Fe-MO protein
contribute
the
from
purified
constitutive
preparations plant
proposed
that contain
to those
constitutive to trypsin
organisms
which
can fix
the constitutive
reported component
component.
by Ketchum in
these
dinitrogen
and Sevilla cells
is
or which
Dialysis (14)
dialyzable
experi-
demonstrate and is
in-
and protease. MATERIALS
AND METHODS
Micrococcus denitrificans ATCC 19367 and Pseudomonas denitrificans ATCC -13867 were grown aerobically in peptone-ammonium medium which contained 0.1 gm peptone, 0.5 gm NH4C1, 0.36 gm Na2HP04, 0.1 gm KH2PO4, 3 mg M&04. 7H20, 0.6 mg FeS04 and 2.0 mg CaC12 per 100 ml of distilled water. Bacillus cereus ATCC 11950, Bacillus licheniformis ATCC 94458, BacillusGbtilis -and Bacillus thurengiensis ATCC 10792 were grown aerobica-on NYB medium (0.8 gm nutrient broth, 0.3 gm yeast extract per 100 ml of distilled water). Rhizobium japonicum ATCC 10324 was grown aerobically on NH4-arabinose-glycerol medium (15). Azotobacter vinelandii was grown Cells were aerobically on Burks medium containing 0.5% casamino acids.
1451
Vol. 52, No. 4, 1973
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
washed twice and then resuspended in 0.02M Na2HP04/NaH2P04 buffer pH 6.5 containing 10m4M Na2MoO4 in a ratio of three volumes of buffer to one gm wet weight of cell. These cell suspensions were passed through a French Pressure Cell at 20,000 lb/in2. The supernatant obtained by centrifugation at 20,000 3 for 20 minutes is designated the crude extract. Crude extracts of nitrate induced --nit-l were prepared as previously described (14). Nitrate reductase and MVH-nitrate reductase were assayed according to the procedures of Garrett and Nason (6). One unit of nitrate reductase equals one nmole nitrite formed per 10 minutes at room temperature. The specific activity of the constitutive component in bacterial extracts was determined as previously described (14). Dialysis tubing (flatwidth of 0.75 inches) was obtained from Fisher Scientific Co. and was prepared by boiling it in sodium bicarbonate, EDTA and then twice in distilled water. Dialysis experiments were performed by adding bacterial crude extracts to 13 x 150 mm test tubes which contained enough glass beads to bring the level of the crude extract outside the dialysis sac to the level of the --nit-l extract inside the dialysis sac. The dialysis sac containing a crude extract of --nit-l was inserted into the tube containing the bacterial extract and the experiment was incubated at room temperature. Aliquots were removed from inside the dialysis Trichlorsac at timed intervals and assayed for NADPH-nitrate reductase. oacetic acid (TCA) soluble protein was determined by measuring the amount of protein by (OD28O/GD260) after precipitating the insoluble protein by making the preparation 5% TCA. NADPH-nitrate reductase is reported as units/ml of the --nit-l extract. RESULTS Extracts
of all
component
which
reductase. extracts crude
participates
in
of Bacillus
2.
component
treatment.
activity
hour.
This
wild
type 2.
Cell
free
MVH-nitrate
is
wild
extracts reductase respectively contained
type g.
in these
contrast
crassa
the --in vitro
extracts
which
(not
more than
after
centrifugation
constitutive
is particulate
specific shown).
hydrogenase
crassa
constitutive
of NADPH-nitrate component
than (9).
that
in crude
observed
The activity
was observed
without
70 per
of the
prior
cent
acid
of the
at 144,000 component
in
a
confor
one
in uninduced
(9).
of g. denitrificans with
greater
extract
to the
the
formation
of the constitutive
was soluble in
1) contained
was 4 to 7 times
In each bacterial
stitutive
(Table
activity
of uninduced
constitutive
vinelandii
tested
The specific
extracts
protein
the bacteria
and -Ps. activities Extracts
as measured
1452
denitrificans of 159.0
of RJ&.
contained and 5.8 units/mg
japonicum
by the methyl
and Azoto.
viologen
re-
Vol. 52, No. 4, 1973
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Vol. 52, No. 4, 1973
duction
method
was observed in place
of Kleiner in
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
and Burris
(13).
the above hydrogenase
of hydrogen
NADPH-nitrate of --nit-l
BIOCHEMICAL
assay
viologen
when nitrogen
reduction
gas was used
gas.
reductase
against
No methyl
was formed
during
of -Ps.
denitrificans
extracts
the dialysis (Fig..
of crude 1).
extracts
Protease
and
Time (minutes) FIGURE 1: Time course of the --in vitro formation of NADPH-nitrate reductase during the dialysis of --nit-l against extracts of -*Ps -de* .-me. , control nitrificans. Three experiments are shown: with no additions; B x--x, 1.0 mg protease/l.5 ml of Ps. denitrificans extract added at time zero; C o-o, 1.0 mg trypzn/l.5 ml of Ps. denitrificans added at time zero. The amount of TCA soluble protein increased from 0 to 14.1% of the total protein present in the Ps. denitrificans extract after 120 minutes i-evueriment B and from 0 to 24.6% in experiment C, (Table 1).
trypsin ulated
digestion
of the --Ps
the formation
constitutive
component
contradiction due to the fact
of NADPH-nitrate is
to a previous that
denitrificans
the
extract reductase
insensitive
to these
report
(9).
complementing
1454
This activity
during
dialysis
demonstrating
that
proteolytic
enzymes
contradiction in -nit-l -)
stim-
is is
the in
probably extremely
Vol. 52, No. 4, 1973
sensitive when
BIOCHEMICAL
to trypsin,
the trypsin
When trypsin
added
reaction,
nitrate
formed
for
The formation against
the
bacterial
is
shown
in Fig.
dialysis
1.
integrity
Trypsin
except stimulated
exception
of protease
ment of extracts amount
(Table
of trypsin
experiment
dialysis
values
the formation
of NADPH-nitrate
reductase
of w.
of proteolytic
was used.
digestion
occured
dialysis
experiment,
protease with
the
treat-
A significant
the bacterial
Table
in all
Protease
performed.
in
during
reductase
of E. denitrificans. was not
report-
Likewise,
of NADPH-nitrate
iaponicum
serves
to
are
extracts
treatment
also
similar
of the bacterial
formation
(23,000
of nit-l
in curves
120 minute
denitrificans
of NADPH-
membrane.
during
the
the amount
dialysis
(9)
the --in vitro
treatment
the
each 120 minute
the
performed
was determined.
The presence
1) resulted only
not
during
mg/ml,
of the dialysis
when g.
treatment
extract
by 95%.
reductase
were component
of 0.01
during
1; however,
stimulated
experiments,
constitutive
reduced extract
extracts
controls
to the --nit-l
of NADPH-nitrate
ed in Table
ing
directly
in the bacterial
as a control
those
of the
at a concentration
reductase
daltons)
appropriate
sensitivity
is
formation
and that
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
extracts
dur-
1.
DISCUSSION The in vitro extracts nit-l rate
of NADPH-nitrate
of the nitrate (9).
The other
uninduced containing experiments
i.e. activities
reductase wild
g.
reported
here
reductase
mutant
of -N. crassa,
formation,
during
in the
four
the
stimulated
flavin
crassa,
(11,12)
specifically
results
appear
enzymes
reductase
one of the
when extracts type
nitrate
in --nit-l
of only
reductase,
nitrate
induced
The mutation
induction,
nitrate (8).
formation
activities
during
(9)
demonstrate
incubated
treated
preparations
of Rhodospirillum that
1455
the
loss
NADPH-
2 reductase
formation with
nit-
with
NADPH-cytochrome
are
acid
or extracts
associated
the --in vitro
of --nit-l
requires
of NADPH-
extracts
of
of molybdenum rubrum
of the
(14).
gene product
The
BIOCHEMICAL
Vol. 52, No. 4, 1973
brought
about
trypsin
and protease
in extracts bolyzing
by the mutation
small
denitrogen
(16)
of
protein is
polypeptide
in E. crassa , nit-l dialyzable
insensitive,
of a selected
sumed to contain
AND BIOPHYSICAL
group
and/or molybdenum
the purification of nitrogenase
which
postulated
our
which
component
be viewed
polypeptide
view
that
the
is
capable
by a present
of metais pre-
as a cofactor
(10,12,14).
of a molybdenum supports
are
The constitutive
and can probably
as previously
can be replaced
component
of bacteria
nitrate.
RESEARCH COMMUNICATIONS
The recent from
or report
the Fe-MO
constitutive
component
a molybdo-polypeptide. ACKNOWLEDGMENT
This work was supported by the National from the Molecular Biology Section.
Science
Foundation
grant
GE-27490
REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16.
Nason, A., and H.J. Evans. 1953. J. Biol. Chem., 202:655-673. Nicholas, D.J.D., A. Nason, and W.D. McElroy, 1954. --J. Biol. Chem. 207:341-351. Nicholas, D.J.D., and A. Nason. 1954. -J. Biol. Chem., 207:353-360. Ibid. , 1954. Z:183-197. Garrett, R.H., and A. Nason. 1967. Proc. Natl. Acad. m. U.S., J&:1603-1610. Garrett, R-H., and A. Nason. 1969. J. Biol. Chem., 244:2870-2882. Sorger, G.J., and N.H. Giles. 1965. Genetics, 52~777-788. Sorger, G.J. 1966. Biochim. Biophys. -.Acta ) U:484-494. Nason, A., A.D. Antoine, P.A. Ketchum, W-A. Frazier III, and D.K. Lee. 1970. Proc. Natl. Acad. u. U.S., 65:137-144. Pateman, J.A., D.J. Cove, B.M. Rever and D.B. Roberts. 1964. Nature -3 -*201.58-60. Ketchum, P.A., H.Y. Cambier, W.A. Frazier III, C.H. Madansky and A. Nason. 1970. Proc. m. Sci -U.S-* 1 E:1016-1023. --Acad -a Nason, A., K.Y. Lee, S.S. Pan, P.A. Ketchum, A. Lamberti and J. DeVries. 1971. Proc. Natl. Acad. Sci. U.S., 68:2242-2246. Kleiner, D. and R.H. Burris. 1970xiochim. zophvs. --Acta 3 212:417-427. Ketchurn, P.A. and C.L. Sevilla. 1973. 2. Bacterial., (in press). Lowe, R. and H. Evans. 1964. Biochim. Biophys. =., 85:377-389. Ganelin, V.L., N.N. L'vov, I.S. Sergeev, G.L. Shanoshnzov and V.L. Kretovich. 1972. DAN SSSR, %:1236-1238.
1456
Vol. 52, No. 4, 1973
--In Vitro
Formation
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
of Assimilatory
of the Constitutive
Nitrate Component
Reductase:
Presence
in Bacteria.
Paul A. Ketchum and Ruth S. Swarin Department of Biological Sciences Oakland University Rochester, Michigan 48063
Received
April
23,
1973 ABSTRACT
Cell-free extracts of a selected group of bacteria which are capable of metabolyzing dinitrogen and/or nitrate contain a soluble form of the constitutive component which is active in the --in vitro formation of NADPH-nitrate reductase when mixed with extracts of N. crassa The constitutive component in these extracts is-dialyzabie --nit-l. and is insensitive to trypsin and protease. The constitutive component which substitutes for the absence of the --nit-l gene product in the --in vitro formation of NADPH-nitrate reductase is postulated to be a low molecular weight cofactor or polypeptide and is shown to be present in a number of unrelated bacteria. INTRODUCTION The Neurospora
assimilatory
oxidoreductase,
E.C.1.6.6.2.)
heteromultimeric
protein,
chrome 557 fied
(l-6).
evidence
flavin suggests
of NADPH-nitrate the
flavin
(9),
have
by mixing contains wild
type
at least
reductase
stimulated
the
four
in -*N
crassa,
The component
contributed
from
associated
with
-N. -3crassa
mutants
of 2.
uninduced
reductase
in the
one of which (7,8).
of NADPH-nitrate
-c reductase,
the
involved
at least
reductase which
with
extracts
extracts
other
and
Genetic formation codes
for
Nason et al.,
nit-l --2
crassa
puri-
NADPH-(FAD)-cyto-
reductase.
c reductase
induced
reductase
and cyto-
(MVH) nitrate
are
dalton,
molybdenum
reductase,
genes
formation
of nitrate
230,000
(FADH2) nitrate
the NADPH-(FAD)-cytochrome or nitrate
are
viologen
NADPH-cytochrome
demonstrated
flavin,
activities
dinucleotide
that
extracts
contains
methyl
(NADPH-nitrate:
inducible
NADPH-nitrate
reduced
adenine
reductase
a nitrate
enzymatic
reductase:
chrome -c reductase, reduced
is which
Four
NADPH-nitrate
NADPII-nitrate
--in vitro specifically of uninduced
than -nit-l --
to the --in vitro
BIOCHEMICAL
Vol. 52, No. 4, 1973
formation
of NADPH-nitrate
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
reductase
is
called
the
constitutive
compon-
ent. Pateman
et al.,
"common
cofactor"
in Aspergillus
nidulans
nitrate
reductase
and xanthine
dehydrogenase
(11)
(10)
demonstrated
that
enzymes
xanthine
tribute
the
nitrate
reductase
oxidase,
nitrate
enzymes
with
the
constitutive
Nason et al.,
(11,12). that
Acid
the
oxidase,
formation
have been
In explaining
can also of NADPH-
containing
shown
these
constitutive
treated
reductase
the known molybdenum
component
nitrate,
similar the
sensitive
to the --in vitro
con-
of NADPH-
sulfite
nitrate
(13)
oxidase
formation treated.
both
containing
and aldehyde
acid
a
et al.,
of the molybdenum
respiratory
all
for
Ketchum
nitrogenase),
of hydrogenase
demonstrates
can reduce
that
Therefore
is
necessary
activity.
first
(from
component
postulated
is
there
to contain
observations,
component
is
a moly-
cofactor.
pap'er
ments
are
exception
(12)
which
that
to the --in vitro
and --E. coli
(12).
evidence
dehydrogenase
enzymes
the constitutive reductase
This
these
reductase
nitrate
bdenum
xanthine component
if
genetic
preparations
of the Fe-MO protein
contribute
the
from
purified
constitutive
preparations plant
proposed
that contain
to those
constitutive to trypsin
organisms
which
can fix
the constitutive
reported component
component.
by Ketchum in
these
dinitrogen
and Sevilla cells
is
or which
Dialysis (14)
dialyzable
experi-
demonstrate and is
in-
and protease. MATERIALS
AND METHODS
Micrococcus denitrificans ATCC 19367 and Pseudomonas denitrificans ATCC -13867 were grown aerobically in peptone-ammonium medium which contained 0.1 gm peptone, 0.5 gm NH4C1, 0.36 gm Na2HP04, 0.1 gm KH2PO4, 3 mg M&04. 7H20, 0.6 mg FeS04 and 2.0 mg CaC12 per 100 ml of distilled water. Bacillus cereus ATCC 11950, Bacillus licheniformis ATCC 94458, BacillusGbtilis -and Bacillus thurengiensis ATCC 10792 were grown aerobica-on NYB medium (0.8 gm nutrient broth, 0.3 gm yeast extract per 100 ml of distilled water). Rhizobium japonicum ATCC 10324 was grown aerobically on NH4-arabinose-glycerol medium (15). Azotobacter vinelandii was grown Cells were aerobically on Burks medium containing 0.5% casamino acids.
1451
Vol. 52, No. 4, 1973
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
washed twice and then resuspended in 0.02M Na2HP04/NaH2P04 buffer pH 6.5 containing 10m4M Na2MoO4 in a ratio of three volumes of buffer to one gm wet weight of cell. These cell suspensions were passed through a French Pressure Cell at 20,000 lb/in2. The supernatant obtained by centrifugation at 20,000 3 for 20 minutes is designated the crude extract. Crude extracts of nitrate induced --nit-l were prepared as previously described (14). Nitrate reductase and MVH-nitrate reductase were assayed according to the procedures of Garrett and Nason (6). One unit of nitrate reductase equals one nmole nitrite formed per 10 minutes at room temperature. The specific activity of the constitutive component in bacterial extracts was determined as previously described (14). Dialysis tubing (flatwidth of 0.75 inches) was obtained from Fisher Scientific Co. and was prepared by boiling it in sodium bicarbonate, EDTA and then twice in distilled water. Dialysis experiments were performed by adding bacterial crude extracts to 13 x 150 mm test tubes which contained enough glass beads to bring the level of the crude extract outside the dialysis sac to the level of the --nit-l extract inside the dialysis sac. The dialysis sac containing a crude extract of --nit-l was inserted into the tube containing the bacterial extract and the experiment was incubated at room temperature. Aliquots were removed from inside the dialysis Trichlorsac at timed intervals and assayed for NADPH-nitrate reductase. oacetic acid (TCA) soluble protein was determined by measuring the amount of protein by (OD28O/GD260) after precipitating the insoluble protein by making the preparation 5% TCA. NADPH-nitrate reductase is reported as units/ml of the --nit-l extract. RESULTS Extracts
of all
component
which
reductase. extracts crude
participates
in
of Bacillus
2.
component
treatment.
activity
hour.
This
wild
type 2.
Cell
free
MVH-nitrate
is
wild
extracts reductase respectively contained
type g.
in these
contrast
crassa
the --in vitro
extracts
which
(not
more than
after
centrifugation
constitutive
is particulate
specific shown).
hydrogenase
crassa
constitutive
of NADPH-nitrate component
than (9).
that
in crude
observed
The activity
was observed
without
70 per
of the
prior
cent
acid
of the
at 144,000 component
in
a
confor
one
in uninduced
(9).
of g. denitrificans with
greater
extract
to the
the
formation
of the constitutive
was soluble in
1) contained
was 4 to 7 times
In each bacterial
stitutive
(Table
activity
of uninduced
constitutive
vinelandii
tested
The specific
extracts
protein
the bacteria
and -Ps. activities Extracts
as measured
1452
denitrificans of 159.0
of RJ&.
contained and 5.8 units/mg
japonicum
by the methyl
and Azoto.
viologen
re-
Vol. 52, No. 4, 1973
BIOCHEMICAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Vol. 52, No. 4, 1973
duction
method
was observed in place
of Kleiner in
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
and Burris
(13).
the above hydrogenase
of hydrogen
NADPH-nitrate of --nit-l
BIOCHEMICAL
assay
viologen
when nitrogen
reduction
gas was used
gas.
reductase
against
No methyl
was formed
during
of -Ps.
denitrificans
extracts
the dialysis (Fig..
of crude 1).
extracts
Protease
and
Time (minutes) FIGURE 1: Time course of the --in vitro formation of NADPH-nitrate reductase during the dialysis of --nit-l against extracts of -*Ps -de* .-me. , control nitrificans. Three experiments are shown: with no additions; B x--x, 1.0 mg protease/l.5 ml of Ps. denitrificans extract added at time zero; C o-o, 1.0 mg trypzn/l.5 ml of Ps. denitrificans added at time zero. The amount of TCA soluble protein increased from 0 to 14.1% of the total protein present in the Ps. denitrificans extract after 120 minutes i-evueriment B and from 0 to 24.6% in experiment C, (Table 1).
trypsin ulated
digestion
of the --Ps
the formation
constitutive
component
contradiction due to the fact
of NADPH-nitrate is
to a previous that
denitrificans
the
extract reductase
insensitive
to these
report
(9).
complementing
1454
This activity
during
dialysis
demonstrating
that
proteolytic
enzymes
contradiction in -nit-l -)
stim-
is is
the in
probably extremely
Vol. 52, No. 4, 1973
sensitive when
BIOCHEMICAL
to trypsin,
the trypsin
When trypsin
added
reaction,
nitrate
formed
for
The formation against
the
bacterial
is
shown
in Fig.
dialysis
1.
integrity
Trypsin
except stimulated
exception
of protease
ment of extracts amount
(Table
of trypsin
experiment
dialysis
values
the formation
of NADPH-nitrate
reductase
of w.
of proteolytic
was used.
digestion
occured
dialysis
experiment,
protease with
the
treat-
A significant
the bacterial
Table
in all
Protease
performed.
in
during
reductase
of E. denitrificans. was not
report-
Likewise,
of NADPH-nitrate
iaponicum
serves
to
are
extracts
treatment
also
similar
of the bacterial
formation
(23,000
of nit-l
in curves
120 minute
denitrificans
of NADPH-
membrane.
during
the
the amount
dialysis
(9)
the --in vitro
treatment
the
each 120 minute
the
performed
was determined.
The presence
1) resulted only
not
during
mg/ml,
of the dialysis
when g.
treatment
extract
by 95%.
reductase
were component
of 0.01
during
1; however,
stimulated
experiments,
constitutive
reduced extract
extracts
controls
to the --nit-l
of NADPH-nitrate
ed in Table
ing
directly
in the bacterial
as a control
those
of the
at a concentration
reductase
daltons)
appropriate
sensitivity
is
formation
and that
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
extracts
dur-
1.
DISCUSSION The in vitro extracts nit-l rate
of NADPH-nitrate
of the nitrate (9).
The other
uninduced containing experiments
i.e. activities
reductase wild
g.
reported
here
reductase
mutant
of -N. crassa,
formation,
during
in the
four
the
stimulated
flavin
crassa,
(11,12)
specifically
results
appear
enzymes
reductase
one of the
when extracts type
nitrate
in --nit-l
of only
reductase,
nitrate
induced
The mutation
induction,
nitrate (8).
formation
activities
during
(9)
demonstrate
incubated
treated
preparations
of Rhodospirillum that
1455
the
loss
NADPH-
2 reductase
formation with
nit-
with
NADPH-cytochrome
are
acid
or extracts
associated
the --in vitro
of --nit-l
requires
of NADPH-
extracts
of
of molybdenum rubrum
of the
(14).
gene product
The
BIOCHEMICAL
Vol. 52, No. 4, 1973
brought
about
trypsin
and protease
in extracts bolyzing
by the mutation
small
denitrogen
(16)
of
protein is
polypeptide
in E. crassa , nit-l dialyzable
insensitive,
of a selected
sumed to contain
AND BIOPHYSICAL
group
and/or molybdenum
the purification of nitrogenase
which
postulated
our
which
component
be viewed
polypeptide
view
that
the
is
capable
by a present
of metais pre-
as a cofactor
(10,12,14).
of a molybdenum supports
are
The constitutive
and can probably
as previously
can be replaced
component
of bacteria
nitrate.
RESEARCH COMMUNICATIONS
The recent from
or report
the Fe-MO
constitutive
component
a molybdo-polypeptide. ACKNOWLEDGMENT
This work was supported by the National from the Molecular Biology Section.
Science
Foundation
grant
GE-27490
REFERENCES 1. 2. 3. 4. 5. 6. 7. 8. 9. 10. 11. 12. 13. 14. 15. 16.
Nason, A., and H.J. Evans. 1953. J. Biol. Chem., 202:655-673. Nicholas, D.J.D., A. Nason, and W.D. McElroy, 1954. --J. Biol. Chem. 207:341-351. Nicholas, D.J.D., and A. Nason. 1954. -J. Biol. Chem., 207:353-360. Ibid. , 1954. Z:183-197. Garrett, R.H., and A. Nason. 1967. Proc. Natl. Acad. m. U.S., J&:1603-1610. Garrett, R-H., and A. Nason. 1969. J. Biol. Chem., 244:2870-2882. Sorger, G.J., and N.H. Giles. 1965. Genetics, 52~777-788. Sorger, G.J. 1966. Biochim. Biophys. -.Acta ) U:484-494. Nason, A., A.D. Antoine, P.A. Ketchum, W-A. Frazier III, and D.K. Lee. 1970. Proc. Natl. Acad. u. U.S., 65:137-144. Pateman, J.A., D.J. Cove, B.M. Rever and D.B. Roberts. 1964. Nature -3 -*201.58-60. Ketchum, P.A., H.Y. Cambier, W.A. Frazier III, C.H. Madansky and A. Nason. 1970. Proc. m. Sci -U.S-* 1 E:1016-1023. --Acad -a Nason, A., K.Y. Lee, S.S. Pan, P.A. Ketchum, A. Lamberti and J. DeVries. 1971. Proc. Natl. Acad. Sci. U.S., 68:2242-2246. Kleiner, D. and R.H. Burris. 1970xiochim. zophvs. --Acta 3 212:417-427. Ketchurn, P.A. and C.L. Sevilla. 1973. 2. Bacterial., (in press). Lowe, R. and H. Evans. 1964. Biochim. Biophys. =., 85:377-389. Ganelin, V.L., N.N. L'vov, I.S. Sergeev, G.L. Shanoshnzov and V.L. Kretovich. 1972. DAN SSSR, %:1236-1238.
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