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p -Hydroxybenzoate hydroxylase: Conformational changes in crystals of holoenzyme vs holoenzyme-substrate complex
BIOCHEMICAL
Vol. 34, No. 1, 1969
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
E-HYDROXYBENZOATE HYDROXYLASE: CONFORMATIONAL CHANGES IN CRYSTALS OF HOLOENZYME -VS HOLOENZYME-SUBSTRATE COMPLEX Keiji Department
Received
November
Yano,
of Agricultural University
hydroxybenzoates
some detail.
and requires
shown
to form 1966).
al., putida tion
addition
complex
FAD but are
attributed
Pseudomonas
holoenzyme-substrate
complex. with
in the visible
absorption
and differences
region
suggest
in the
followed
previously
reported
Protein from
(Yario
substrate
change
in the
protein.
the holoenzyme
of 68,000.
was determined
P. desmolytica
et al.,
1966).
substrate
according
procedures
in the ultrabinding. NADPH oxidato Kalcker,
IAM 1123 cultured All
in addition.
in sedimentation
dispersion
on the
and the
The molecule
shift
rotatory
hydroxy-
on ultracentrifuga-
by the -p-hydroxybenzoate-dependent
at 340 my-
The enzyme was prepared
by the
1 mole of the substrate
change
The absorp-
region
a slight
et
Pseudomonas
1966).
are homogeneous
was
(Katagiri
of p-hydroxybenzoate
weight
optical
1965)
from
et al.,
namely
spectrum,
a conformational
The enzyme was assayed tion
a molecular
1 mole of FAD and the complex
coefficient violet
Both forms
et al.,
FAD and salicylate
forms
in
FAD as the prosthetic
hydroxylase
IAM 1123,
hydroxylases
and investigated
(Yamamoto
to a conformational two crystalline
and electrophoresis
Changes
donor
in the visible
desmolytica
two bacterial
contains
NADPH (Hosokawa
changed
lase
contains
which
p-hydroxybenzoate
slightly
we have prepared
studied,
of apoenzyme,
requires
Recently,
tion
of Agriculture Japan
to homogeneity
NADH as the electron
and were
from
purified
hydroxylase
The crystalline
spectra
Chemistry, Faculty of Tokyo, Tokyo 113,
have been
a ternary
contains
and Kei Arima
monooxygenases
Salicylate
group
Higashi
1, 1968
Among the flavoprotein for
Naoki
for
1947.
by the method the preparation
Vol. 34, No. 1, 1969
were
BIOCHEMICAL AND BIOPHYSKAL
done at 0 - 5*C.
M succinate
buffer,
were
pH 6.0,
mercaptoethanol. stated.
Cells
containing
The same buffer
A clear
supernatant
at 100,000
sulfate
and centrifuged
to remove
through
a DEAE-Sephadex
A-25
(0.35
volume
x g for
- 0.60
of the buffer,
fractions
were
enzyme was eluted eluate
with
about
excess Fine
yellow
tallization
was done
recognized
G-25
column
sulfate
to remove
a slightly
holoenzyme
reduced
which
concentrations
were
enzyme forms
phoresis.
A typical
molecular (Yphantis, activity
weight
were
that
the
was calculated
Since
and the
substrate. Recryshere
were
in Fig.
through
addition
a Sephadex
of ammonium
was kept
in a desiccator
more than
3 days.
The crystals
the
increase
and the protein
partial
to be 68,000
is summarized volume
by the short
specific The number
2
(Fig.
activity
of
of the 2).
on ultracentrifugation
specific
1.
in a minimum
solution
with
the
The enzyme
obtained
and passed
procedure
to be 2700.
washing,
chloride,
of the
was dissolved
appeared
the maximal
Active
and are shown
After
homogeneous
purification
was estimated
1960).
rods
in a minimum
a few minutes.
complex
ammonium sulfate
crystalline
On the assumption
for
frac-
to be a slightly
The crystals
substrate.
yellowish
of both
within
complex
pressure
was passed
After
M sodium
in the presence
the
it
of protamine
filtration.
was brought
appeared
saturation,
of the
ammonium sulfate.
mercaptoethanol
the bound
to make a 0.55
under
0.15
same manner.
containing
gel
column.
with
holoenzyme-substrate
of the buffer
Then
A-50
to be the holoenzyme-substrate
The crystalline volume
in the
otherwise
0.1 volume
G-100
concentration,
crystals
unless
was dissolved
containing
of ammonium sulfate
and 1 mM
by an ammonium sulfate
by a Sephadex
by precipitation
needle-shaped
with
followed
in 0.017
centrifugation
the precipitate.
the buffer
oscillator
steps
by the
The precipitate
a 3 W protein
saturation
all
was treated
on a DEAE-Sephadex
was concentrated
solution,
obtained
column,
followed
applied
a sonic
was used for
30 min.
satn.).
with
0.1 mM p-hydroxybenzoate
fluid
sonicate
tionation
disrupted
RESEARCH COMMUNICATIONS
Both and electro-
in Table
I.
was 0.75
ml/g,
column
method
was 40, the molecular
of FAD molecule
was computed
BIOCHEMICAL
Vol. 34, No. 1, 1969
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Fig.
Fig.
to be 0.9 by assuming that for
of free NADPH.
FAD. Optimun
that
the molar
The -Km values pH was 8.2
extinction
were to 8.6.
3
25 PM for
1. Crystalline substrate
holoenzymecomplex.
2. Crystalline
of bound
holoenzyme.
FAD is
p-hydroxybenzoate
The enzyme reacted
the same as and 40pM
specifically
Vol. 34, No. 1, 1969
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Table
I.
Purification
of p-hydroxybenzoate
Treatment Crude extract Protamine sulfate treatment Ammonium sulfate frac. Sephadex G-100 gel filt. DBAE-Sephadex A-50 column Holoenzyme-substrate complex First crystallization Second crystallization Holoenzyme Second crystallization
with
NADPH and not with
benzoate, tion.
however, Very
observed
with
Total protein
Total activity
Specific activity
yield
ml 1,500 1,650 50 130 100
w 40,000 29,900 4,210 895 160
units 12,000 11,850 9,700 7,650 6,000
units/ml 0.3 0.4 2.3 8.5 37.5
% 100 98.5 80.5 63.2 50.1
3 3
123 97
4,900 3,900
39.8 40.2
40.7 32.3
2
76
3,060
40.0
25.4
highly
specific
NADH, and was also
activities
spectra the
of which
were found
and 2,4-dihydroxybenzoate Absorption
Volume
the concentration
low
(0.9 of both
spectrum
hydroxylase
with
above
to p-hydroxy-
1 mM showed
3,4-dihydroxybenzoate
an inhibi(1.4
%)
%). forms
of the
are
complex
shown in Pig. at 365,
380,
3.
Shoulders
were
430 and 475 rnp, while
Visible absorption spectra of both forms. Concentrations of each enzyme solutions were 260 m)rmoles (19 mg) in 3 ml, at pH 6.0. -; the holoenzyme, -----; the holoenzymesubstrate complex. Hitachi 124 double beam spectrophotometer.
the spectral titration ratio
curve
of the holoenzyme
of the holoenzyme of the holoenzyme
was rather
by E-hydroxybenzoate
: the
substrate
smooth,
Spectrophotometric
at 385 rnr showed
was 1 : 1.1 at pH 6.0.
4
that
the
When the
BIOCHEMICAL
Vol. 34, No. 1, 1969
holoenzyme
was excited
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
at 375 my, a sharp
having
a maximum at 520 rnp was observed.
erable
quenching
of the fluorescence at this
showed
that
above mentioned
strate
complex
ratio
while
was 1 : 0.9.
formed
spectrum
binding,
a consid-
the substrate
Fluorometric
wave length.
was specifically
emmision
On the substrate
occured,
not show any emmision the
fluorescence
titration
Thus
by an equimolar
itself
did
at 520 rn+
the holoenzyme-sub-
holoenzyme
and sub-
strate. Sedimentation of the complex
coefficient, 5.0 S.
performed
in the
two cells
containing
volume
a single
cient
same run
appeared peak.
time really
using
in Schlieren
exists
This
indicates
between
the
larger
pattern case,
was 5.1
than
that
that
and also
centrifuge
with When the
of the complex, and finally
in sedimentation demonstrates
two
fused
of two boundaries
a difference
two forms
were
respectively.
became closer the distance
S and that
experiments
UCA-1A analytical
and the complex,
was slightly
In the reverse
elapsed,
a Hitachi
the holoenzyme
of the holoenzyme
boundaries
with
S20 w, of the holoenzyme , To confirm this small difference,
that
into
increased coeffia small
3a
Fig. 2a ‘b
4. Ultraviolet dispersion hydroxylase.
optical rotatory of p-hydroxybenzoate
Cell chamber was kept an anaerobic condition with nitrogen gas at a slightly positive pressure. The concentration of the enzyme was 0.12 to 0.0022 % at pH 6.0, 22-25'C. The mean residue molecular weight of 115 was employed.
2 IO
-; ------;
the holoenzyme, the holoenzymecomplex.
Japan Spectroscopic ORD/W-5 recording
5
substrate
model polarimeter.
Vol. 34, No. 1, 1969
but
distinct
conformational
An attempt aqueous
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
by the optical
The curve
effect
since
specific
holoenzyme
the
(Cassim
et al.,
1967).
the case of the
complex
from
ed unchanged.
The results
coil
difference
with
that
the
wave length
hindered
shift
% helix
suggest
that
binding
in the p-structure
Crystallization
region
content
could
a-Helix
content
of the complex
in
remain-
change
and/or
might
in a
was observed
conformational
This
of Cotton
to be -8190
of the curve
a small
in
the measurement.
was calculated
to a 47.6
A slight
forms
might
in the random was rather
easy
also
be due to the
was first
reported
in the conformations.
acid
of an enzyme-substrate
oxidase
(Yagi
(molecular
since
it
et al.,
oxygen).
enzyme-substrate
oxygen,
4 has a trough
shorter
(m')232
of the holoenzyme.
Crystallization
acceptor
in the
of both
in the ultraviolet
208 to 225 rnp , however,
of the protein.
as compared
structures
dispersion
corresponds
on the substrate
region
D-amino
value
internal
absorption
value
This
be induced
peak
rotation
was caused.
shown in Fig.
strong
1963).
protein
the rotatory
The positive
not be determined,
(Fasman,
the
of
at 232 mp.
The corrected
of the protein
was made to clarify
solutions
region.
change
1964)
complex
in the absence
of the
electron
In the case of p-hydroxybenzoate
complex
was easily
can not react
with
crystallized
the substrate
even without
with
hydroxylase,
in the
presence
electron
donor,
of
NADPH. A rather D-amino
acid
et al.,
1967).
large
reduction
oxidase
It
Very
small
(Yankeelov
a complex
benzoate,
shift
was found
that
enzyme which
protein
moiety.
The details
The authors wish Paul's University,
1965),
had not drawn
p-hydroxybenzoate might
with
was induced
et al.,
of ultracentrifugation
present
St.
coefficient
on forming
phosphoglucomutase two runs
in sedimentation
be a result will
plays
was reported an inhibitor
by the substrate however,
in this
a role
in the case of case,
separate
as an activator
in a subsequent
to express their sincere thanks to Prof. discussion. Tokyo , Japan for his useful
6
(Yagi
a conclusion.
of the conformational
be described
with
change
of the of the
paper. T. Kimura, The
Vol. 34, No. 1, 1969
BIOCHEMCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
authors also indebted to Dr. E. Ichijima and Mr. K. Hayashi, Central Research Institute, Kikkoman Shoyu Co., Noda, Japan, for their kind help in ultraviolet optical rotatory dispersion measurements. References Cassim, Fasman,
J.Y. and Yang, J-T., Biochem. Biophys. Res. Comm., 26, 58 (1967). G.D. in "Methods in Enzymology" Vol. 6, Pd. by Colozck, S.P. and Kaplan, N.O., Academic Press, New York (1963), p. 928. Hosokawa, K. and Stanier, R.Y., J. Biol. Chem., 241, 2453 (1966). Kalcker, H.M., J. Biol. Chem., 167, 461 (1947). Katagiri, M., Takemori, S., Suzm, K. and Yasuda, H., J. Biol. Chem., 241, 5675 (1966). Yagi, K. and Ozawa, T., Biochim. Biophys. Acta, 81, 29 (1964). Yagi, K., Naoi, M., Harada, M., Okamura, K., Hidaka, H., Ozawa, T. and Kotaki, A., J. Biochem. (Tokyo), 61, 580 (1967). Yamamoto, S., Katagiri, M., Maeno, H. and Hayaishi, O., J. Biol. Chem., 240, 3408 (1965). Yano, K., Morimoto, M. and Arima, K., Agr. Biol. Chem (Tokyo), 30, 91 (1966). Yphantis, D.A., Ann. New York Acad. Sci., E, 586 (1960).
Vol. 34, No. 1, 1969
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
E-HYDROXYBENZOATE HYDROXYLASE: CONFORMATIONAL CHANGES IN CRYSTALS OF HOLOENZYME -VS HOLOENZYME-SUBSTRATE COMPLEX Keiji Department
Received
November
Yano,
of Agricultural University
hydroxybenzoates
some detail.
and requires
shown
to form 1966).
al., putida tion
addition
complex
FAD but are
attributed
Pseudomonas
holoenzyme-substrate
complex. with
in the visible
absorption
and differences
region
suggest
in the
followed
previously
reported
Protein from
(Yario
substrate
change
in the
protein.
the holoenzyme
of 68,000.
was determined
P. desmolytica
et al.,
1966).
substrate
according
procedures
in the ultrabinding. NADPH oxidato Kalcker,
IAM 1123 cultured All
in addition.
in sedimentation
dispersion
on the
and the
The molecule
shift
rotatory
hydroxy-
on ultracentrifuga-
by the -p-hydroxybenzoate-dependent
at 340 my-
The enzyme was prepared
by the
1 mole of the substrate
change
The absorp-
region
a slight
et
Pseudomonas
1966).
are homogeneous
was
(Katagiri
of p-hydroxybenzoate
weight
optical
1965)
from
et al.,
namely
spectrum,
a conformational
The enzyme was assayed tion
a molecular
1 mole of FAD and the complex
coefficient violet
Both forms
et al.,
FAD and salicylate
forms
in
FAD as the prosthetic
hydroxylase
IAM 1123,
hydroxylases
and investigated
(Yamamoto
to a conformational two crystalline
and electrophoresis
Changes
donor
in the visible
desmolytica
two bacterial
contains
NADPH (Hosokawa
changed
lase
contains
which
p-hydroxybenzoate
slightly
we have prepared
studied,
of apoenzyme,
requires
Recently,
tion
of Agriculture Japan
to homogeneity
NADH as the electron
and were
from
purified
hydroxylase
The crystalline
spectra
Chemistry, Faculty of Tokyo, Tokyo 113,
have been
a ternary
contains
and Kei Arima
monooxygenases
Salicylate
group
Higashi
1, 1968
Among the flavoprotein for
Naoki
for
1947.
by the method the preparation
Vol. 34, No. 1, 1969
were
BIOCHEMICAL AND BIOPHYSKAL
done at 0 - 5*C.
M succinate
buffer,
were
pH 6.0,
mercaptoethanol. stated.
Cells
containing
The same buffer
A clear
supernatant
at 100,000
sulfate
and centrifuged
to remove
through
a DEAE-Sephadex
A-25
(0.35
volume
x g for
- 0.60
of the buffer,
fractions
were
enzyme was eluted eluate
with
about
excess Fine
yellow
tallization
was done
recognized
G-25
column
sulfate
to remove
a slightly
holoenzyme
reduced
which
concentrations
were
enzyme forms
phoresis.
A typical
molecular (Yphantis, activity
weight
were
that
the
was calculated
Since
and the
substrate. Recryshere
were
in Fig.
through
addition
a Sephadex
of ammonium
was kept
in a desiccator
more than
3 days.
The crystals
the
increase
and the protein
partial
to be 68,000
is summarized volume
by the short
specific The number
2
(Fig.
activity
of
of the 2).
on ultracentrifugation
specific
1.
in a minimum
solution
with
the
The enzyme
obtained
and passed
procedure
to be 2700.
washing,
chloride,
of the
was dissolved
appeared
the maximal
Active
and are shown
After
homogeneous
purification
was estimated
1960).
rods
in a minimum
a few minutes.
complex
ammonium sulfate
crystalline
On the assumption
for
frac-
to be a slightly
The crystals
substrate.
yellowish
of both
within
complex
pressure
was passed
After
M sodium
in the presence
the
it
of protamine
filtration.
was brought
appeared
saturation,
of the
ammonium sulfate.
mercaptoethanol
the bound
to make a 0.55
under
0.15
same manner.
containing
gel
column.
with
holoenzyme-substrate
of the buffer
Then
A-50
to be the holoenzyme-substrate
The crystalline volume
in the
otherwise
0.1 volume
G-100
concentration,
crystals
unless
was dissolved
containing
of ammonium sulfate
and 1 mM
by an ammonium sulfate
by a Sephadex
by precipitation
needle-shaped
with
followed
in 0.017
centrifugation
the precipitate.
the buffer
oscillator
steps
by the
The precipitate
a 3 W protein
saturation
all
was treated
on a DEAE-Sephadex
was concentrated
solution,
obtained
column,
followed
applied
a sonic
was used for
30 min.
satn.).
with
0.1 mM p-hydroxybenzoate
fluid
sonicate
tionation
disrupted
RESEARCH COMMUNICATIONS
Both and electro-
in Table
I.
was 0.75
ml/g,
column
method
was 40, the molecular
of FAD molecule
was computed
BIOCHEMICAL
Vol. 34, No. 1, 1969
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Fig.
Fig.
to be 0.9 by assuming that for
of free NADPH.
FAD. Optimun
that
the molar
The -Km values pH was 8.2
extinction
were to 8.6.
3
25 PM for
1. Crystalline substrate
holoenzymecomplex.
2. Crystalline
of bound
holoenzyme.
FAD is
p-hydroxybenzoate
The enzyme reacted
the same as and 40pM
specifically
Vol. 34, No. 1, 1969
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
Table
I.
Purification
of p-hydroxybenzoate
Treatment Crude extract Protamine sulfate treatment Ammonium sulfate frac. Sephadex G-100 gel filt. DBAE-Sephadex A-50 column Holoenzyme-substrate complex First crystallization Second crystallization Holoenzyme Second crystallization
with
NADPH and not with
benzoate, tion.
however, Very
observed
with
Total protein
Total activity
Specific activity
yield
ml 1,500 1,650 50 130 100
w 40,000 29,900 4,210 895 160
units 12,000 11,850 9,700 7,650 6,000
units/ml 0.3 0.4 2.3 8.5 37.5
% 100 98.5 80.5 63.2 50.1
3 3
123 97
4,900 3,900
39.8 40.2
40.7 32.3
2
76
3,060
40.0
25.4
highly
specific
NADH, and was also
activities
spectra the
of which
were found
and 2,4-dihydroxybenzoate Absorption
Volume
the concentration
low
(0.9 of both
spectrum
hydroxylase
with
above
to p-hydroxy-
1 mM showed
3,4-dihydroxybenzoate
an inhibi(1.4
%)
%). forms
of the
are
complex
shown in Pig. at 365,
380,
3.
Shoulders
were
430 and 475 rnp, while
Visible absorption spectra of both forms. Concentrations of each enzyme solutions were 260 m)rmoles (19 mg) in 3 ml, at pH 6.0. -; the holoenzyme, -----; the holoenzymesubstrate complex. Hitachi 124 double beam spectrophotometer.
the spectral titration ratio
curve
of the holoenzyme
of the holoenzyme of the holoenzyme
was rather
by E-hydroxybenzoate
: the
substrate
smooth,
Spectrophotometric
at 385 rnr showed
was 1 : 1.1 at pH 6.0.
4
that
the
When the
BIOCHEMICAL
Vol. 34, No. 1, 1969
holoenzyme
was excited
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
at 375 my, a sharp
having
a maximum at 520 rnp was observed.
erable
quenching
of the fluorescence at this
showed
that
above mentioned
strate
complex
ratio
while
was 1 : 0.9.
formed
spectrum
binding,
a consid-
the substrate
Fluorometric
wave length.
was specifically
emmision
On the substrate
occured,
not show any emmision the
fluorescence
titration
Thus
by an equimolar
itself
did
at 520 rn+
the holoenzyme-sub-
holoenzyme
and sub-
strate. Sedimentation of the complex
coefficient, 5.0 S.
performed
in the
two cells
containing
volume
a single
cient
same run
appeared peak.
time really
using
in Schlieren
exists
This
indicates
between
the
larger
pattern case,
was 5.1
than
that
that
and also
centrifuge
with When the
of the complex, and finally
in sedimentation demonstrates
two
fused
of two boundaries
a difference
two forms
were
respectively.
became closer the distance
S and that
experiments
UCA-1A analytical
and the complex,
was slightly
In the reverse
elapsed,
a Hitachi
the holoenzyme
of the holoenzyme
boundaries
with
S20 w, of the holoenzyme , To confirm this small difference,
that
into
increased coeffia small
3a
Fig. 2a ‘b
4. Ultraviolet dispersion hydroxylase.
optical rotatory of p-hydroxybenzoate
Cell chamber was kept an anaerobic condition with nitrogen gas at a slightly positive pressure. The concentration of the enzyme was 0.12 to 0.0022 % at pH 6.0, 22-25'C. The mean residue molecular weight of 115 was employed.
2 IO
-; ------;
the holoenzyme, the holoenzymecomplex.
Japan Spectroscopic ORD/W-5 recording
5
substrate
model polarimeter.
Vol. 34, No. 1, 1969
but
distinct
conformational
An attempt aqueous
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS
by the optical
The curve
effect
since
specific
holoenzyme
the
(Cassim
et al.,
1967).
the case of the
complex
from
ed unchanged.
The results
coil
difference
with
that
the
wave length
hindered
shift
% helix
suggest
that
binding
in the p-structure
Crystallization
region
content
could
a-Helix
content
of the complex
in
remain-
change
and/or
might
in a
was observed
conformational
This
of Cotton
to be -8190
of the curve
a small
in
the measurement.
was calculated
to a 47.6
A slight
forms
might
in the random was rather
easy
also
be due to the
was first
reported
in the conformations.
acid
of an enzyme-substrate
oxidase
(Yagi
(molecular
since
it
et al.,
oxygen).
enzyme-substrate
oxygen,
4 has a trough
shorter
(m')232
of the holoenzyme.
Crystallization
acceptor
in the
of both
in the ultraviolet
208 to 225 rnp , however,
of the protein.
as compared
structures
dispersion
corresponds
on the substrate
region
D-amino
value
internal
absorption
value
This
be induced
peak
rotation
was caused.
shown in Fig.
strong
1963).
protein
the rotatory
The positive
not be determined,
(Fasman,
the
of
at 232 mp.
The corrected
of the protein
was made to clarify
solutions
region.
change
1964)
complex
in the absence
of the
electron
In the case of p-hydroxybenzoate
complex
was easily
can not react
with
crystallized
the substrate
even without
with
hydroxylase,
in the
presence
electron
donor,
of
NADPH. A rather D-amino
acid
et al.,
1967).
large
reduction
oxidase
It
Very
small
(Yankeelov
a complex
benzoate,
shift
was found
that
enzyme which
protein
moiety.
The details
The authors wish Paul's University,
1965),
had not drawn
p-hydroxybenzoate might
with
was induced
et al.,
of ultracentrifugation
present
St.
coefficient
on forming
phosphoglucomutase two runs
in sedimentation
be a result will
plays
was reported an inhibitor
by the substrate however,
in this
a role
in the case of case,
separate
as an activator
in a subsequent
to express their sincere thanks to Prof. discussion. Tokyo , Japan for his useful
6
(Yagi
a conclusion.
of the conformational
be described
with
change
of the of the
paper. T. Kimura, The
Vol. 34, No. 1, 1969
BIOCHEMCAL
AND BIOPHYSICAL RESEARCH COMMUNICATIONS
authors also indebted to Dr. E. Ichijima and Mr. K. Hayashi, Central Research Institute, Kikkoman Shoyu Co., Noda, Japan, for their kind help in ultraviolet optical rotatory dispersion measurements. References Cassim, Fasman,
J.Y. and Yang, J-T., Biochem. Biophys. Res. Comm., 26, 58 (1967). G.D. in "Methods in Enzymology" Vol. 6, Pd. by Colozck, S.P. and Kaplan, N.O., Academic Press, New York (1963), p. 928. Hosokawa, K. and Stanier, R.Y., J. Biol. Chem., 241, 2453 (1966). Kalcker, H.M., J. Biol. Chem., 167, 461 (1947). Katagiri, M., Takemori, S., Suzm, K. and Yasuda, H., J. Biol. Chem., 241, 5675 (1966). Yagi, K. and Ozawa, T., Biochim. Biophys. Acta, 81, 29 (1964). Yagi, K., Naoi, M., Harada, M., Okamura, K., Hidaka, H., Ozawa, T. and Kotaki, A., J. Biochem. (Tokyo), 61, 580 (1967). Yamamoto, S., Katagiri, M., Maeno, H. and Hayaishi, O., J. Biol. Chem., 240, 3408 (1965). Yano, K., Morimoto, M. and Arima, K., Agr. Biol. Chem (Tokyo), 30, 91 (1966). Yphantis, D.A., Ann. New York Acad. Sci., E, 586 (1960).