The phospholipase D (PLD) was purified from leaves of cabbage (Brassica oleracea L. var. capitata L.) . The molecular weight of the enzyme was estimated as ...
(33)
Food
Preservation
Science
VOL.
25
NO.5
1999
(Article〕
229
Transphosphatidylation capacity of phospholipase D from cabbage (Brassica oleracea L. var. capitata L.) leaves and Streptomyces chromofuscust WATANABE Toshihiro *, SATO Hiroaki *, NAKAZAWA Yozo * *, SAGANE Yoshimasa * KOZIMAT. Tsuneo * and TAKANO Katsumi * * * Department of Food Science, Faculty of Bioindustry, Tokyo University of Agriculture 196, Yasaka, A bashiri -shi, Hokkaido 099-2493 * * Department of Applied Biology and Chemistry, Faculty of Applied Bioscience, Tokyo University of Agriculture 1-1-1, Sakuragaoka, Setagaya - ku, Tokyo 156-8502
The phospholipase D (PLD) was purified from leaves of cabbage (Brassica oleracea L. var. capitata L.) . The molecular weight of the enzyme was estimated as 87 and 73.5-kDa on SDS-PAGE and gel filtration using Superdex 200 HR 10/30 column. The transphosphatidylation capacity of cabbage PLD was shown to be higher than that of Streptomyces chromofuscus PLD. Although cabbage PLD showed a single band, Streptomyces chromofuscus PLD gave several bands on nondenaturing and denaturing PAGE. These results indicated that the cabbage PLD was a monomer protein, while the Streptomyces chromofuscus PLD was hetero oligomer, having several types with different molecular weights. Furthermore, the cabbage PLD included the duplicated HxKxxxxD catalytic motifs in the molecule, but the Streptomyces chromofuscus PLD did not. Previously, YAMANE et al. reported that the transphosphatidylation capacity of Streptomycessp. PLD was higher than that of Streptomyces chromofuscus. These results indicated that the high degree of the transphosphatidylation capacity of cabbage PLD was due to the existence of HxKxxxxD catalytic motifs. (Received Jul. 21, 1999 ; Accepted Jul. 23, 1999)
In
recent
years,
the
development
of
novel
alcohol.
phospholipids was attempted in the oil and fat industries. Especially, phosphatidylcholine (PC )
it
obtained as a by-product during purification of oil and fat or from yolk lecithin is widely used.
(PG)
Phospholipase
D (PLD; EC 3.1.4.4) hydrolyzes
This
possible
(PE)
from
catalyzes
capacity
of
phospholipase
D
II
YANG
that
activity
have to
PC, and
et
al.4)
and
and
phosphatidylglycerol (PC)
superior they
are
PLD
purified
pharmaceutical DAWSON5)
from
the
transphosphatidylation
Thereafter,
PLD
from
these
microorganisms
and
for
oil
and
fat
industry.1)•`3) reported They
catalyzed
. Since
solubility useful
transphosphatidylation. the
makes
phosphatidylethanolamine (PS)
phosphatidylcholine
dispersibility
Further, the enzyme catalyzes not only degradation
†Transphosphatidylation
synthesize
phospholipids
manufacturing
phospholipids, but also transphosphatidylation transferring a phosphatidyl group to primary hydroxyl groups in the presence of primary
to
, phosphatidylserine
phospholipids at the phosphorus diester bond, leading to the formation of phosphatidic acid (PA) . of
transphosphatidylation
leaves
that
PLD
demonstrated of
cabbage of
was
PC. shown
230
Food Preservation Science VOL. 25 NO. 5 1999
to
catalyze
genus
transphosphatidylation.
Streptomyces
was
transphosphatidylation YAMANE
et
transphosphatidylation
chromofuscus
PLD
Streptomyces
sp.
HxKxxxxD
motifs
PLD
of
in
activity.
of
lower
than
al.13)
amino
Streptomyces
that
chromofuscus
was
we
will
capacity
of
the
cabbage
of
that
degree
with
a
lacking
of
Branson
Co.,
motifs.
In
this
conditions. of
having
HxKxxxxD
CaC12,
L.
cv.
)
from
(Str.)
a
Louis,
MO,
99.1%
produced
PC
and
0.4%
reagents
used
D Co.
the
lecithin
emulsion
carried
out
lyophilized
of
PLD
of
PLD
as
) .
purchased City,
leaves
precipitation
CA,
grade
the t
.
reaction
LoNG.15) by
LAMBRECHT ABOUSALHAM
procedure PLD
the
and et
was
methods
ULBRICH
.
from
. All
other
was
adding
0.2me
50mM
EDTA.
distilled
10mt
)
was 450,
ice
cold
of
0.1me
40mM of
enzyme
5min,
by
the
adding
0.1me
The
at
500nm.
reaction
as
and
from
described
described purified
by from
the
16)
and
reported -
HOFMANN
curve
obtained
filtration an
Pharmacia,
spectrophotometrically
test,
0.1me
of
the
of
1% was
distilled
choline
of the
amount was
way
absorbance
absorbance using
and
same of
the
the
standard of
choline
defined
produced
conditions
30
solution,
in
known
that
the
2me
amount
PLD
for
density
enzyme
the
a
adding
of
as
the
1,umol
described
of
above.
filtration
Gel on
by
of
was
37•Ž
optical
sample,
of
phenol, at
treated
enzyme
under
of
from
the
unit
the
choline/min
by
of
,umol
The
with
One of
unit ,umol
the
subtracting that
8.0)
mixture,
1.5
calculated
by from
4 .Gel
was
of
1.5
the
of
(pH
1.2me
containing
blank
above. was
blank
amount
a
instead
at was
peroxidase,
stopped
mixture
chloride.
acetone
As
used
incubated
Tris-HC1
incubated
and
and
mixture
this
2.1
was X-100,
was
of
was
mixture
was
0.5M To
and
Triton
read
of
unit
mixture
a substrate,
reaction
water 0.2
The
obtained
prepared
al .17).
assayed
0.1ne . After
as
the
aminoantipyrine
the
crude
min,
oxidase,
water
was
Briefly,
assay activity
and 37•Ž
(1.0me)
by
of
(w/v)
U.S.A.) was
leaves
coagulation
the
in
reaction
mixture 10
int
min.
leaves
cabbage
was
heat
at
After
added.
Mini
commercially
cabbage
from
powder by
and
precipitate
from
reported14).
using
DAVIDSON
PLD
(w/v)
choline
from
R -250
highest
previously
acetone
cabbage
3. PLD
1%
liberated
Purification
water
started
4-
available. 2.Purification
U.S.A.)
containing
was
0.4
( St.
containing
Switzerland)
the
distilled
in
Sonifier
composed
mixture
stopped
was
(CBB)
(Buchs, of
PC-98S
8.0)
preincubated
containing
phospholipase
Japan
were ( Foster
were
was
Chemical
( Tokyo,
Blue
AG
of
of
emulsion
(0.9me) (pH
was
37
Streptomyces
(PC-98S,
Co.
Brilliant Chemie
capitata
lysophosphatidylcholine)
Biosystems
Coomassie
var.
Hokkaido
sp.
. Lecithin
membranes
Applied
Fluka
Str.
Sigma
Q.P.
ProBlottTM
in
and
from
L.
market.
from U.S.A.)
obtained
oleracea
vegetable
chromofusucus purchased
CT,
- HCl
maximal
Methods
(Brassica
Kinsyun
obtained
were
0.7me
a lecithin
(model;
mixture
Tris
peroxidase
solution
sonicator
solution
then cabbage
yolk 100mg
Danbury,
The
20mM
coupled
by
deoxycholate a
to
oxidatively phenol
Egg
was
simultaneous
with
500nm.
sodium
prepared
to
was
concentration,
mM
the
chromophore at
HORIUTi18).
oxidation
with
and
a
of
Materials Fresh
which
(w/v) 40
of 1.
of
give
of
transphosphatidylation
and
oxidase
H2O2,
and generated
after
choline
absorbance (1%
low
Imamura choline
4-aminoantipyrine
to
of
motifs.
Materials
by
with
the
sequences
by
free
colorimetrically,
production
that
method of
capacity due
PLD
modified
amount
betaine
Streptomyces
the
catalytic
discuss
a
The
phosphatidylalchol
inferred
HxKxxxxD
paper,
using
that
reported acid
in
We
reported
transphosphatidylation
duplicated
from superior
estimated
capacity
et the
involved
the
have
al.12)
was
PONTING
were
synthase
to
capacity.6)•`11)
Previously, the
PLD
reported
(34)
chromatography
AKTA
system Uppsala,
Superdex
200
calibrated
with
HR
was ( model
Sweden 10
/
thyroglobulin
30
; )
carried
equipped
( Pharmacia (669-kDa)
out
Purifier
900, with
)
column , ferritin
a
(35)
〔Article〕
Transphosphatidylation
capacity
( 440- kDa ) , aldolase ( 158- kDa ) , bovine serum albumin ( 67- kDa ) , ovalbumin ( 43- kDa ) and ribonuclease A (13.7- kDa ) as molecular weight standards (Pharmacia) . Proteins were eluted with 30mM PIPES buffer (pH 6.7) containing 50mM CaC12 and 0.15M NaCl at a constant flow rate of 0.25ml/min. 5.Polyacrylamide gel electrophoresis Nondenaturing (PAGE) by
polyacrylamide
was
performed
ORNSTEIN 19 of
resolving
phase
6.8)
in
the
to
gel
soaked
was
containing
-HCI
and
(pH
overnight The
8.0) and
the
w
stained
v
(pH
30min
crushed
was
in and
6.8)
( pH
the
then 0.7mg
of
was
PLD
and
gel,
containing
extracted
with
then
0.125M
band
. After
(pH 6.8) containing 0.1% (w/v) SDS, overnight. The eluted protein was concentrated, and then subjected to reducing SDS-PAGE. SDS-PAGE was performed with a 15% (w/v) acrylamide gel as described by LAEMMLI 21 ). Protein samples containing 10mM Tris-HC1 (pH 6.8) , 1% (w/v) SDS, 1% (v/v) 2-mercaptoethanol and 20% (v/v)
as
analyze
the
mixture.
with
The
in a proper on Chromarod
silica
gel
attached
pH 8.0, cabbage;
pH
.
performed by the et al .22). Thin layer ionization detector Analyzer new MK
was used to in the samples
of chloroform
were
rods
coated Tokyo,
micropipettes (1-3ƒÊl)
of
a
sample were
spotted glass
rods tank
( acetone
together spotted
having
in first
acid,
the
rods
were
from
the
bottom
developing
then
scanned.
The
An aliquot standards
the
of
chromarods.
a frame
were
put
developing
70
: 0.25,
were
v
burned
and
into
solvent / v
) .
again
developed
solvent
After
leaving again
with
(chloroform-acetone-
acid-distilled
transferred
with on
enclosed
- acetic
development, 20mm
Disposable
were used for spotting. each
phospholipids The
to the integrator.
the rods with
(Str. chromofuscus;
37•Ž
Japan ) . Just before use, the blank rods were activated by passing them through the flame of the
by heating
Tris-HC1
then
at
Laboratories,
development,
of 0.1ml of 20mM
1%
and
incubated
S III quartz
( Iatron
v/v) . After
(0.9ml) composed
of
evaporated
quantity
methanol-acetic
of phospholipids
mixture
quantitatively
(w/v) CBB R-250 and then destained.
The mixture
the 0.1ml
substrate,
Co., Kyoto, Japan)
phospholipids
6.Transphosphatidylation extraction
a was
second
and
adding
(1.0ml
glycerol were boiled for 5 min. After electrophoresis the gels were stained with 0.25% reaction
5min,
by
enzyme
Laboratories Co., Tokyo, Japan) with an integrator (model; Chromatopac
TLC/FID
Tris-HC1
of
concentrations
The reaction was stopped by adding 0.2ml of 1N HCl. To this 1.2me of mixture, 5.0 ml of Folch solution (chloroform-methanol, 2:1) and 0.9ml of distilled water was added. After mixing well, the solution was centrifuged for 5min at 2500r.p.m. and the lower layer was collected and the extractions were evaporated with a vacuum rotary evaporator. The evaporated samples were dissolved in a proper quantity of chloroform. 7. Phospholipids analysis
spotted in
(w/v) the
37•Ž
0.1 ml
desired
started
mixture
dissolved
with Each
0.1%
and
the
emulsion
reaction
reaction
soaked
at was
lecithin
CaC12,
to
C-R6A, Shimadzu .
activity.
destained. the
equilibrium,
4•Ž
stained
reaction
connected
Tris
at
preincubated
the (w/v)
mM
glycerol
was
the
40
and
-5 ,Iatron
slice
CaC1 2, left
briefly
excised
)
direction
2mM
containing
solution
231
D
Phospholipids analysis was methods described by JUNEJA chromatography with a frame (TLC/FID) (model; Iatroscan
into
each
4 mM
for
8.0
cut
centrifugation
R -250
band
Tris-HC1 for
to
assayed gel
a
then the
was
and
by
the CBB
protein
0.125M SDS
hand,
and
- HC1 lane
containing
were
other
0.25%
Tris
with
removed
a
at
electrophoresis,
Each
extracted
run
min
perpendicular
supernatant
On
30
migration,
crushed
the
using
was
for
2 mM
slices
gel in
(pH
performed
. After
CaCl2.
slab 8.9)
acrylamide
gel
V
4•Ž
in
electrophoretic
was
was
at
4mM 1.6mm
80
described The (pH
and, The
of
120V
methods 20 ).
(w/v)
phase
system.
increased
electrophoresis
acrylamide 3.5%
stacking
voltage
the
DAVIS
(w/v) and
constant
of
and
7.5%
discontinuous
serial
by
)
consisted
gel
7.0)
of phospholipase
water,
6.5: 2: 1: 1: 0.3,
the solvent was removed a hot dryer. to
TLC / FID
the was
The rods
instrument conducted
and at
a
232•@
Food
Preservation
Science
hydrogen gas flow rate of 160ml/min, an air flow rate of 200ml/min and a scanning speed of 40 sec/ scan. The concentration of PC, PG and PA were estimated from their peak areas with the help of the integrator. Results 1 . Purification of cabbage PLD on chromatography PLD from cabbage leaves was fractionated by acetone precipitation from crude extract. The precipitate was dissolved in 30mM PIPES buffer (pH 6.2) containing 50mM CaCl2, and subjected to an Octyl Sepharose CL -4 B ( Pharmacia )
VOL.25
NO.5
1999•@(
hydrophobic with by
36
chromatography
the
same
stepwise
buffer. gradient
fraction
of
containing
against
20mM
applied
to
Tris
Mono
HR
chromatography buffer.
linear
M).
Elution
are
shown
gradient
The of
profiles in
equilibrated was
dialyzed
( pH
7.5 ),
(Pharmacia) column
absorbed NaCl
The
was
buffer 5/5
performed
concentration.
activity
equilibrated
PLD
by
and anion
was
concentration
obtained
Fig.
2. Determination
CaCl2
- HC1
Q
with a
elution
PLD
exchange same
column
The
eluted (0•`0.5
chromatography
I. of
molecular
weight
on
gel
filtration Purified
PLD
was
concentrated
(A)
(B)
Fig. 1 Elution profiles of PLD from cabbage leaves on Octyl Sepharose CL-4B column and Mono Q HR 5/5 column
)
to
minimum
by
(37)
Transphosphatidylation
〔Article〕
volume by using VIVAPORE 10/20 (Viva Science Limited, Binbrook, U.K.) , and applied to Superdex 200 HR 10 / 30 ( Pharmacia ) column equilibrated with 30mM PIPES buffer (pH 6.7) containing 50mM CaCl2 and 0.15 M NaCl. The
capacity
of phospholipase
233
D
elution was performed with a flow rate of 0.25ml/ min. As a result, the molecular weight of cabbage leaves PLD was estimated as approximately 73.5kDa by retention volumes relative to protein standards as shown in Fig. 2. 3 . Electrophoretic analysis Cabbage, Str. sp. and Str. chromofuscus PLD
Fig. 2
Calibration
of molecular
weight of purified
PLD from cabbage leaves Proteins were applied to Superdex 200 HR 10/30 (bed volume, 24 ml, Vt ) equilibrated with 30 mM PIPESbuffer (pH6.7) containing 50 mM CaC12 and 0.15 M NaCl. The protein standards gave a linear plot of log molecular weight versus Kay ( (Ve-Vo)/(VtVia),V0 was determined by using blue dextran 2000). Other conditions are described in Materials and Methods.
A. nondenaturing
Fig.
3
Comparison
strain, resolved 1 ;cabbage leaves, loaded onto 7.5% in the presence
PAGE
of separation
preparations were subjected to nondenaturing PAGE by the method of ORNSTEIN19)and DAVIS20) using 7.5% (w/v) acrylamide gels. As shown in Fig. 1, on nondenaturing PAGE, cabbage and Str. sp. PLD demonstrated only one band, While Str. chromofuscus PLD gave five protein bands (Fig. 3). On SDS-PAGE, cabbage and Str. sp. PLD gave one band with a molecular mass of approximately 87 and 67- kDa, on the other hand, Str. chromofuscus PLD yielded five peptide bands with molecular masses of approximately 57, 40, 18, 17 and 14-kDa. The nondenaturing PAGE gel of Str. chromofuscus PLD was sliced at intervals of 1.6mm parallel to the protein bands. Protein in the gel slices was extracted into 2mM Tris- HC1 buffer (pH 8.0) containing 4mM CaCl2. The PLD activity of each extract was measured. As shown in Fig.
B. SDS- PAGE
patters
of
PLD
from
different
on nondenaturing PAGE and SDS-PAGE 2; Str. sp., 3; Str. chromofuscus. (A)Each protein was polyacrylamide gel. (B) Each protein was boiled for 5 min of 2- mercaptoethanol, and loaded onto 15% SDS -
polyacrylamide gel, M; molecular standards (97kDa ; phosphorylase b, 64 kDa ; bovine serum albumin, 43 kDa ; ovalbumin, 30 kDa ; carbonic anhydrase, 20.1kDa ; try psin inhibitor, 14.4kDa ; a - lactalbumin)
Fig.
4
Nondenaturing
chromofuscus Protein
( 100 ƒÊg
acrylamide elution gel
was
PAGE
separation
of
Str.
PLD
gel. were sliced
/ lane PAGE
described (1.6mm)
)
was
loaded
conditions in
Materials
and
assayed
onto and
7.5%
method and for
( w / v )
of protein
Methods. PLD
The
activuty.
234•@
Food
Fig.
5
SDS-PAGE
protein M
Preservation
separation
band molecular
serum
albumin,
kDa;
trypsin
PLD,
N1,
slices
N2,
(94 kDa
43kDa;
ovalbumin,
N4
and
PAGE
gel (7.5% of
2-
N5 to
acrylamide).
Str.
25
NO.
b,
protein and
and
67 kDa
carbonic
lactalbumin),
position
(38)
each
PAGE
30kDa;
Each
mercaptoethanol,
1999•@
PLD
; phosphorylase
; proteins, the
5
chromofuscus
nondenaturing
14.4kDa; ƒ¿-
corresponded
presence acrylamide
on
standards
N3,
VOL.
of
resolved
inhibitor,
that
Science
S;
Str.
respectively, of
was
on
boiled
loaded
from
gel
nondenaturing for
onto
20.1
chromofuscus
eluted
bands
; bovine
anhydrase,
5 min
15%
in the
(w
/ v )
gel.
4, these proteins separated on nondenaturing PAGE demonstrated PLD activity. N1 showed the highest activity. The five native Str. chromofuscus PLDs with different molecular sizes, obtained by nondenaturing PAGE, were subjected to SDS PAGE using 15% (w/v) acrylamide gels. As shown in Fig. 5, these proteins were separated into several polypeptides with molecular masses of 57, 40, 18, 17 and 14- kDa, although the molecular ratios of these polypeptide were different from each other. This result indicated that native Str. chromofuscus PLD was formed by association of several polypeptides with different molecular masses. 4 . Transphosphatidylation capacity
from
these
maximum cabbage
values.
As
shown
transphosphatidylation
in
Fig.
6,
capacities
the of
was more than 90% in 5% (w/v) glycerol,
whereas,
that
of Str. chromofuscus
PLD was 46.89
% in 20% (w/v) glycerol. These results indicated that cabbage PLD had a high affinity to glycerol and
low
compared
transphosphatidylation
capacity
with Str. chromofuscus.
The transphosphatidylation capacities of cabbage and Str. chromofuscus PLD preparations were measured using egg yolk PC as the substrate in the presence of 0, 5, 10, 15, 20 and 30% (v/v) glycerol. PC as a substrate and the PG and PA as products were isolated by TLC. The areas of spots on TLC were measured using TLC/FID, and the transphosphatidylation capacity was calculated
Fig. 6 The transphosphatidylation capacity of PLD from cabbage and Streptomyces chromofuscus in the presence of glycerol at various concentrations
(39)•@
(Article)
Transphosphatidylation
capacity
of
phospholipase
D•@
235
Fig. 7 Alignment of deduced amino acid sequences of PLD from cabbage (two isozymesof PLD1 and PLD2, respectively, designated by PANNENBERG et al.)23), Streptornyces sp.24)and Streptornyces chromofuscus25).Dashes indicate breaks inserted to maximize algnments using the multiple alignments program Clustal W26). The conserved histidine, lysine and aspartic acid residues in the duplicated HxKxxxxD catalytic motifs involving phosphatidylserine synthase and cardiolipin synthase from Escherichia coli13) are indicated by boxes.
Food Preservation Science VOL. 25 NO. 5 1999
236
∼
Discussion The PLD was purified from extract of cabbage leaves by acetone precipitate, hydrophobic chromatography and anion-exchange chromatography. The molecular weight of purified enzyme was estimated as 87 and 73.5- kDa on SDS - PAGE and gel filtration, indicating the enzyme was a monomer. The Str. chromofuscus PLD preparation was separated into five protein bands on nondenaturing PAGE. These proteins had PLD activities. SDSPAGE analysis of these proteins clarified that these were hetero-oligomers formed by association of several polypeptides with noncovalent bonds. These results indicated that the native Str. chromofuscus PLD had several types of oligomers comprised of several polypeptide with different molecular weights. The transphosphatidylation capacities of Str. chromofuscus and cabbage PLD were compared. The maximum transphosphatidylation capacity and affinity to glycerol of Str. chromofuscus PLD was lower than those of cabbage PLD. Previously, YAMANE et al.12) reported that the transphosphatidylation capacity of Str. chromofuscus PLD was lower than that of Str. sp. PONTING et al.13) reported that the HxKxxxxD motifs in the amino acid sequence of PLD were involved in phosphatidylalchol synthase activity. As shown in Fig. 7, although duplicated HxKxxxxD motifs were observed in sequences of PLD from cabbage23) and Str. sp.24),they were not in the sequence of Str. chromofuscus PLD25). These results indicated that the differences in amino acid sequences, especially lack of HxKxxxxD motifs, might be involved in the differences in transphosphatidylation capacity of PLD. It was considered that the cabbage PLD was useful for development of phospholipid due to the high degree of transphosphatidylation capacity. References 1) D'ARRIGO, P. and SERVI, S. : Trends Biotechnol., 15, 90-96 (1997) 2) WANG, P., SCHUSTER, M., WANG, Y-F. and WONG, C-H. : J. Am. Chem. Soc., 115, 10487
(40 )
10490 (1993)
3) HIDANO, N., KAMATA, M., HARA, S. and TOTANI, Y. : J. Jpn. Oil Chem. Soc., 44, 49-55 (1995) 4) YANG, S. F., FREER, S. and BENSON, A. A. : J. Biol. Chem., 242, 477-484 (1967) 5) DAWSON,R. M. C. Biochem. J., 102, 205-210 (1967) 6) JUNEJA, L. R., KAZUOKA,T., YAMANE,T. and SHIMIZU,S.: Biochirn. Biophys. Acta., 960,334 ∼
341 (1988)
7) JUNEJA, L. R., KAZUOKA, T.,
GOTO, N.,
YAMANE, T. and SHIMIZU, S. : Biochim. Biophys. Acta., 1003, 277-283 (1989) 8) IWASAKI,Y., NAKANO, H. and YAMANE,T. : Appl. Microbiol. Biotechnol., 42, 290 299 (1994) 9) NAKAJIMA, J., NAKASHIMA, T. and. SHIMA, Y. : Biotechnology and Bioengineering, 44, 1193 ∼ 10)
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CARREA,
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4681
起 源PhospholipaseDの
chromofuscus
ホ ス フ ァチ ジ ル 基
転移能の比較
PLDよ
り も高 か
よびSDS-PAGE上
Streptomyces PAGEお
で単 一 で あ っ た。 しか し、
chrornofuscus のPLDは
よびSDS-PAGEに
、nondenaturing
お い て い くつ か の バ ン ド
を 与 え た。 こ の 結 果 はStyeptornyces
chromofuscus
品 に は い くつ か の ポ リペ プ チ ドの会 合 に よ っ て
形 成 さ れ た い くつ か のヘ テ ロ 多量 体 が 存 在 す る こ とを示 唆 した。 ま た 、先 に 報 告 さ れ て い る キ ャ ベ ツ 起 源PLDと Streptomyces
chromofuscus
PLDの
ア ミ ノ酸 配 列 を比
較 した。 キ ャベ ツ起 源PLDに
はN末 端 よ り330残 基 近 傍
と660残 基 近 傍 にPONTINGら
に よってホスフ ァチ ジル
ア ル コー ル 合 成 酵 素 に 関 与 す る こ と が 示 唆 さ れ た HxKxxxxDモ
チ ー フ の 存 在 が 確 認 さ れ た。 一 方 、
Streptomyces
chyoynofuscus起
源
の そ れ
に は
チー フ に類 似 した配 列 が 存 在 して い た も
の の、 本 モ チー フ の存 在 は確 認 で きなか っ た。 先 にYAMANEら
は 、Streptomyces属
由来PLDは
優れ
た ホ ス フ ァ チ ジ ル基 転 移 能 を有 す る もの のStreptomyces
(PhospholipaseDの ホ ス フ ァチ ジル 基 転移 能 に 関 す る研 究 第2報)
chromofuscus由
来PLDを
用 いた場合、転移 反応はほ と
ん ど進 行 しな い こ とを見 出 した。 ま た、 彼 ら は転 移 能 の 高 いPLDの
渡 部 俊 弘*・ 佐 藤 広 顕*・ 中 澤 洋 三**・ 相 根 義 昌*
ア ミ ノ酸 配 列 は そ の タ ン パ ク質 全 体 に お い
て相 同性 が 高 い こ とを報 告 して い る。 こ れ らの こ とか ら、 キ ャベ ツ 起 源PLDの
小 嶋 秩 夫*・ 高 野 克 己** * 東京農 業 大学 生物 産業 学部 食 品科 学科 (〒099-2493北
chrornofuscus
キ ャ ベ ツ の 葉 か ら精 製 さ れ たPLDはnondenaturing
HxKxxxxDモ キ ャ ベ ツ 葉 お よびStreptornyces
237
D
ジ ル基 転 移 能 がStyeptornyces
ホ ス フ ァチ
chrornofuscus
PLDそ
の
そ れ よ り高 い こ と は ア ミ ノ 酸 配 列 の 差 異、 特 に
海 道 網 走 市 八 坂196)
** 東 京 農 業 大 学 応 用 生 物 科 学 部 生 物 応 用 化 学 科
HxKxxxxDモ
(〒156-8502東
れ た。 こ れ らの事 実 は タ ンパ ク工 学 的 手 法 か らの 追 究 に
京 都 世 田 谷 区 桜 丘1-1-1)
チ ー フ の 有 無 に 起 因 す る こ とが 考 え ら
よ り確 実 に 証 明 され るだ ろ う。 さ ら に 、 キ ャベ ツ起 源 本 論 文 で は起 源 の 異 な るPhospholipaseD
(PLD)
の ホ ス フ ァ ジル 基転 移 能 を比 較 し、 さ らに そ の 電 気 泳 動
PLDは
、 そ の優 れ た ホ ス フ ァ ジ ル 基 転 移 能 よ り、 リン
脂 質 の改 良 に適 した試 料 で あ る と考 え られ た。
法 に よ る解 析 、 そ して 先 に 報 告 され た全 ア ミノ酸 配 列 を 比較 ・検 討 した。 キ ャベ ツ の葉 か ら精 製 され たPLDの
(平成11年7月21日 ホ スフ ァジル基
受付
平 成11年7月23日
受 理)
