J Biol Chem, Vol. 274, Issue 35, 24503-24513, August 27, 1999
-Oxidation of Fatty Acids in Higher Plants
IDENTIFICATION OF A PATHOGEN-INDUCIBLE OXYGENASE (PIOX) AS AN
-DIOXYGENASE AND BIOSYNTHESIS OF 2-HYDROPEROXYLINOLENIC ACID*
Mats
Hamberg
§,
Ana
Sanz¶, and
Carmen
Castresana¶
From the Division of Physiological Chemistry II,
Department of Medical Biochemistry and Biophysics, Karolinska
Institutet, S-171 77 Stockholm, Sweden and the ¶ Centro Nacional
de Biotecnología, CSIC, Campus Universidad Autónoma,
Cantoblanco, E-28049 Madrid, Spain
 |
ABSTRACT |
A pathogen-inducible oxygenase in
tobacco leaves and a homologous enzyme from Arabidopsis
were recently characterized (Sanz, A., Moreno, J. I., and
Castresana, C. (1998) Plant Cell 10, 1523-1537). Linolenic
acid incubated at 23 °C with preparations containing the recombinant
enzymes underwent -oxidation with the formation of a chain-shortened
aldehyde, i.e.,
8(Z),11(Z),14(Z)-heptadecatrienal (83%), an -hydroxy acid,
2(R)-hydroxy-9(Z),12(Z),15(Z)-octadecatrienoic acid (15%), and a chain-shortened fatty acid,
8(Z),11(Z),14(Z)-heptadecatrienoic acid (2%). When incubations were performed at 0 °C,
2(R)-hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic acid was obtained as the main product. An intermediary role of 2(R)-hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic
acid in -oxidation was demonstrated by re-incubation experiments, in
which the hydroperoxide was converted into the same -oxidation
products as those formed from linolenic acid.
2(R)-Hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic acid was chemically unstable and had a half-life time in buffer of
about 30 min at 23 °C. Extracts of cells expressing the recombinant oxygenases accelerated breakdown of the hydroperoxide (half-life time,
about 3 min at 23 °C), however, this was not attributable to the
recombinant enzymes since the same rate of hydroperoxide degradation
was observed in the presence of control cells not expressing the
enzymes. No significant discrimination between enantiomers was observed
in the degradation of
2(R,S)-hydroperoxy-9(Z)-octadecenoic acid in the presence of recombinant oxygenases. A previously studied system for -oxidation in cucumber was re-examined using the newly developed techniques and was found to catalyze the same conversions as
those observed with the recombinant enzymes, i.e. enzymatic -dioxygenation of fatty acids into 2(R)-hydroperoxides
and a first order, non-stereoselective degradation of hydroperoxides into -oxidation products. It was concluded that the recombinant enzymes from tobacco and Arabidopsis were both
-dioxygenases, and that members of this new class of enzymes
catalyze the first step of -oxidation in plant tissue.
| |
INTRODUCTION |
Fatty acid hydroperoxides serve as important intermediates in the
oxylipin pathway of fatty acid oxygenation in plants and fungi (1-4).
Further metabolism of the hydroperoxide derivatives of linoleic and
linolenic acids results in the formation of fatty acid epoxides and
epoxy alcohols (5-7), dihydroxy acids (8, 9), short-chain aldehydes
(10, 11), and divinyl ethers (12-15). One specific hydroperoxide
isomer, i.e. the 13(S)-hydroperoxide derivative
of linolenic acid, is converted into jasmonic acid by a series of
reactions catalyzed by allene oxide synthase, allene oxide cyclase,
reductase, and 
-oxidation enzymes (2). This pathway is of biological
importance in plants because it produces compounds which are involved
in defense reactions against insects and other phytopathogens (16), in
mechanical responses such as tendril coiling (17), and pollen
development (18).
A variety of conditions, such as mechanical perturbation, osmotic
stress, attack by plant pathogens and wounding, elicit increased formation of jasmonates and other biologically active oxylipins in
plant leaves (19). This is partly a consequence of liberation of free
linolenic acid from its esterified forms (20, 21) but may also depend
on increased levels of enzymes catalyzing hydroperoxide formation and
metabolism. In a recent study, tobacco leaves were found to accumulate
a 75-kDa protein in response to bacterial infection (22). This protein,
as well as a protein from Arabidopsis showing a 75%
homology in amino acid sequence, were expressed in insect cells and
found to cause uptake of molecular oxygen in the presence of
polyunsaturated fatty acids such as linolenic acid, linoleic acid, and
arachidonic acid. Interestingly, the tobacco enzyme, called
"pathogen-inducible oxygenase"
(PIOX),1 showed significant
homology to prostaglandin-endoperoxide H synthases-1 and -2 present in
animal tissue (22).
The present study was carried out with the aim of identifying the
catalytic function of the pathogen-induced oxygenase from tobacco
leaves and its homologous enzyme from Arabidopsis. Evidence will be presented that both enzymes are fatty acid -dioxygenases which catalyze conversion of linolenic acid and other fatty acids into
their 2(R)-hydroperoxy derivatives. The mode of degradation of these unstable hydroperoxides into chain-shortened aldehydes and
other -oxidation products has also been studied.
| |
EXPERIMENTAL PROCEDURES |
Labeled Fatty Acids--
[1-14C]Linolenic,
[1-14C]linoleic, and
[9,10-3H2]oleic acids were purchased from NEN
Life Science Products Inc. (Boston, MA). Dilution with unlabeled
materials (Nu-Chek-Prep, Elysian, MN) followed by purification by
SiO2 chromatography afforded specimens having specific
radioactivities of 8.9, 3.8, and 184 kBq/µmol, respectively. In the
same way, [9,10,12,13,15,16-3H6]linolenic
acid (American Radiolabeled Chemicals, St. Louis, MO) was diluted with
unlabeled linolenic acid and purified to make a specimen having a
specific radioactivity of 22.2 kBq/µmol.
2(R)- and 2(R,S)-Hydroxylinolenic Acid--
Seeds of
Thymus vulgaris (23) were ground in an electric coffee mill
and the powder (25 g) was extracted under an argon atmosphere for
2 h with hexane (250 ml) containing BHT (12 ppm) in a Soxhlet
apparatus. The oil (8.5 g) was subjected to methanolysis and
fractionated by SiO2 open column chromatography. Elution
with diethyl ether/hexane (7:93, v/v) afforded methyl
2-hydroxylinolenate (1.0 g) having a purity of 98% according to GLC
analysis. Treatment with 1 M NaOH in 50 ml of 50% methanol
containing BHT afforded the free acid. The identity of the material
obtained with 2-hydroxylinolenic acid was confirmed by analysis of the
methyl-esterified material by GC-MS. Prominent ions were observed at
m/z 308 (M+; 4% relative intensity), 279 (M+ 
29; loss of ·CH2CH3;
1), 252 (2), 161 (6), 135 (12), 108 (32), 79 (100), 67 (74), and 55 (48). The mass spectrum of the Me3Si derivative of the
methyl ester showed ions at m/z 380 (M+; 3%),
365 (M+ 15; loss of ·CH3; 15), 321 (M+ 59; loss of ·COOCH3; 13), 161 (Me3SiO+ = CH-COOCH3; 10), 159 (14), 89 (Me3SiO+; 40), 79 (52), and 73 (Me3Si+; 100). The stereochemistry of the
hydroxy acid, which was not unequivocally determined in the previous
work (23), was established as "R" by GLC analysis of the
MC derivative of the methyl ester. The percentage of the
2(S) isomer was less than 1%.
2(R,S)-Hydroxylinolenic acid was prepared by reduction of
methyl 2-ketolinolenate (see below) with NaBH4 followed by saponification.
Methyl 2-ketolinolenate--
The methyl ester of
2(R)-hydroxylinolenic acid (31 mg) was oxidized with
chromium trioxide-pyridine complex in methylene chloride (24).
Purification by open column SiO2 chromatography afforded methyl 2-ketolinolenate (12 mg) having a purity in excess of 98%. The
mass spectrum showed prominent ions at m/z 306 (M+; 3%), 250 (2), 247 (M+ 59; loss of
·COOCH3; 2), 187 (3), 159 (7), 93 (50), 79 (100), 67 (81), and 55 (58). The Fourier transform-infrared spectrum (film)
showed absorption bands at 1754 and 1732 cm
1 due to the
ester and keto carbonyls, respectively.
8(Z),11(Z),14(Z)-Heptadecatrienal--
2(R)-Hydroxylinolenic
acid (400 mg) was treated under an argon atmosphere with sodium
periodate (1.5 g) in acetone (40 ml) containing glacial acetic acid (20 ml) and water (10 ml) at 50 °C for 21 h (cf. Ref.
25). The product obtained by extraction with light petroleum (about
80% of aldehyde and 15% of unoxidized hydroxy acid) was subjected to
SiO2 open column chromatography. Elution with diethyl
ether/hexane (5:95, v/v) afforded
8(Z),11(Z),14(Z)-heptadecatrienal (200 mg; purity, 98%). A faint odor of fresh seaweed was noted for the
sample. The Fourier transform-infrared spectrum (film) showed
absorption bands at inter alia 1727 cm1
(aldehyde carbonyl) and 2715 cm1 (C-H stretching in
aldehyde group). The mass spectrum showed prominent ions at
m/z 248 (M+; 2%), 219 (1), 192 (3), 135 (6),
121 (8), 108 (23), 93 (45), 79 (100), 67 (79), and 55 (48). The
O-methyloxime (MO) derivative showed two peaks on GC-MS
analysis due to syn/anti isomerism. The mass spectra
recorded on these peaks were virtually identical and showed prominent
ions at 277 (M+, 0.5%), 262 (M+ 15; loss of
·CH3; 1), 246 (M+ 31; loss of
·OCH3; 21), 190 (7), 166 (7), 108 (23), 93 (42), 79 (100), 67 (75), and 55 (52).
8(Z),11(Z),14(Z)-Heptadecatrienoic Acid--
Mixed fatty acid
methyl esters prepared from the seed oil of T. vulgaris (see
above) were saponified and subjected to RP-HPLC using solvent
system II.
8(Z),11(Z),14(Z)-Heptadecatrienoic
acid (nor-linolenic acid, Ref. 23) appeared with an elution volume of
37.9 ml (linolenic acid, 54.7 ml). The mass spectrum of the methyl
ester showed prominent ions at m/z 278 (M+;
7%), 247 (M+ 31; loss of ·OCH3; 2),
222 (3), 177 (3), 149 (9), 135 (10), 121 (17), 108 (27), 93 (48), 79 (100), 67 (72), and 55 (49).
[9,10-3H2]2(R,S)-Hydroperoxyoleic
Acid--
2-Hydroperoxyoleic acid and 2-hydroperoxypalmitic acid were
prepared by modification of a method previously described (26). For
preparation of the first mentioned compound, butyllithium (0.8 mmol)
was added at 78 °C to an argon-purged solution of diisopropylamine
(0.1 ml) in 1.5 ml of dry tetrahydrofuran. A solution of
[9,10-3H2]oleic acid (111 mg; 25 MBq) and
hexamethylphosphoric triamide (63 µl) in 0.25 ml of tetrahydrofuran
was added and the mixture was kept under argon at 50 °C for 30 min.
The material was added under a period of 30 min to 25 ml of
oxygen-saturated diethyl ether at 78 °C. Oxygen gas was
continuously bubbled into the reaction mixture in order to maintain
oxygen saturation and to effect rapid dispersion of the introduced
oleate dianion. Material obtained by extraction with diethyl ether was
analyzed by RP-HPLC using solvent system IV. Three main peaks were
observed, i.e. 2-hydroperoxyoleic acid (13.0 ml effluent),
2-hydroxyoleic acid (13.8 ml), and oleic acid (27.1 ml). Effluent
containing 2-hydroperoxyoleic acid was collected and rapidly extracted
with diethyl ether. The ether phase was dried over MgSO4
and taken to dryness in vacuo. The residual
2-hydroperoxyoleic acid was dissolved in dry acetone and stored at
25 °C. Analysis of the specimen by radio-HPLC showed a
radiochemical purity in excess of 95%. The specific radioactivity was
32 kBq/µmol (the drop in specific activity compared with that of the
starting material was due to a slight chromatographic separation between ditritio- and unlabeled molecules in the RP-HPLC purification step resulting in partial loss of the 3H2
compound). As expected, the 2-hydroperoxyoleic acid was reducible into
2-hydroxyoleic acid by treatment with SnCl2 or
triphenylphosphine. Furthermore, treatment of the hydroperoxide with
sodium borodeuteride afforded 2-hydroxyoleic acid with no detectable
incorporation of deuterium. An aliquot of the hydroperoxide was treated
with BSTFA and analyzed by GC-MS. Considerable degradation with
formation of 8(Z)-heptadecenal (30%, 6.3 min retention
time), the Me3Si ester of 2-ketooleic acid (9%, 10.2 min),
the Me3Si ether/ester of 2-hydroxyoleic acid (18%, 10.7 min), the Me3Si ether/ester of the enol form of 2-ketooleic
acid (16%, 10.9 min) took place, however, a portion of the
hydroperoxide derivative (27%) chromatographed as the intact
Me3Si peroxide and appeared as a peak at 11.3 min. The mass
spectrum recorded on this material showed prominent ions at
m/z 443 (M+ 15; loss of
·CH3; 1%), 426 (M+ 32; rearrangement
with loss of CH3OH; 9), 341 (M+ 117;
elimination of ·COOSiMe3; 6), 251 (341-90; 3), 163 (Me3Si-O-O+ = SiMe2; 13), 147 (Me3Si-O+ = SiMe2; 27), 89 (Me3SiO+; 53), and 73 (Me3Si+; 100).
Enzyme Preparations--
Recombinant oxygenases were obtained
from insect cells infected with baculovirus carrying pFASTBAC (vector),
pFASTBAC-tob.A5.2, or pFASTBAC-ara.N38086 (22). Cell suspensions in
1-2 ml of sonication buffer (22) were sonicated at 0 °C by four
bursts of 10 s and subsequently centrifuged at 12,000 × g for 6 min. The supernatants (protein, 1-2 mg/ml) were
diluted with 0.1 M potassium phosphate buffer, pH 6.7 or
7.4, and directly used for the incubations. Two crude preparations of
the -oxidation system of cucumber (27-29) were obtained in the
following way. Cucumber fruits were peeled and the flesh and seed parts
(175 g) were diced and added to 0.1 M potassium phosphate
buffer, pH 6.7 or 7.4 (175 ml). The tissue was homogenized at 0 °C
for two periods of 60 s using an Ultra-Turrax and subsequently
filtered through gauze. The filtrate (protein, 0.6-0.7 mg/ml) was
directly used for small scale incubations carried with various fatty
acid substrates. For larger scale incubations carried out in order to
prepare 2-hydroperoxy acids, the filtrate was centrifuged for 15 min at
1,100 × g. The supernatant was decanted and further
centrifuged at 48,000 × g for 30 min. The sediment fraction was either suspended in potassium phosphate buffer (140 ml;
protein, 0.2-0.3 mg/ml) and used for the incubations or frozen and
stored at 25 °C. The 105,000 × g particle
fraction of homogenate of seeds of Vicia faba L. was
prepared as described previously (6). Suspensions of this material in
0.1 M potassium phosphate buffer, pH 6.7 (protein, 0.6 mg/ml), were used as a source of peroxygenase (6).
Incubations--
Incubations of the tobacco and
Arabidopsis oxygenases, and of whole homogenate of cucumber,
were carried out with 50-250 µM fatty acid at 23 or
0 °C for the times indicated. The mixtures were diluted with 1 volume of distilled water, acidified to pH 4, and extracted twice with
diethyl ether. The combined ether phases were washed with water and
taken to dryness in vacuo. In most incubations, the material
obtained was immediately dissolved in HPLC mobile phase, centrifuged,
and analyzed by RP-radio-HPLC. For incubations with peroxygenase,
suspensions (0.5 ml) of the membrane fraction from V. faba
seeds were preincubated at 23 °C for 5 min with the lipoxygenase
inhibitor 5,8,11,14-eicosatetraynoic acid (50 µM).
Subsequently, [9,10-3H2]oleic acid (100 µM) and hydroperoxide (30-264 µM) were
added and stirring continued for 15 min. The reaction products were extracted with diethyl ether, and the material obtained was analyzed by
RP-radio-HPLC.
Preparation of 2(R)-Hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic
Acid--
Linolenic acid (5.9 mg; concentration, 152 µM)
was stirred at 0 °C for 30 min with a suspension (140 ml) of the
48,000 × g particle fraction of homogenate of
cucumber. The mixture was acidified to pH 4 and rapidly extracted with
2 volumes of diethyl ether. The material obtained following evaporation
of the solvent was suspended in HPLC mobile phase (0.4 ml). After
centrifugation, aliquots of 0.1 ml were subjected to RP-HPLC using
solvent system I at a flow rate of 2 ml/min. Effluent containing the
hydroperoxide (37.0-39.4 ml) was immediately extracted with diethyl
ether and the solution dried over MgSO4. Hydroperoxide
obtained from several such incubations was dissolved in 0.5 ml of dry
acetone (concentration, 10 mM) and stored at 25 °C.
The yield of hydroperoxide from the incubated linolenic acid was
5-10% and the radiochemical purity was in excess of 95%. The
identity of the hydroperoxide with
2(R)-hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic acid was based on chemical and spectral analyses as described under
"Results."
Methods for Estimation of the Stability of
2-Hydroperoxides--
The rate of breakdown of 2-hydroperoxides in
enzyme preparations or in buffer was determined by using one of two
methods. In method A, tritium-labeled
2(R)-hydroperoxylinolenic acid (35 µM) was
stirred at 23 °C with enzyme preparation or buffer (0.8 or 1 ml). At
different times of stirring, the sample was directly subjected to
RP-radio-HPLC using a column protected with a pre-column and a solvent
system consisting of acetonitrile/water (80:20, v/v) at a flow rate of
2 ml/min. Remaining hydroperoxide was eluted as its salt (3.6-6.0 ml
effluent), well separated from the main product of hydroperoxide
breakdown, i.e.
8(Z),11(Z),14(Z)-heptadecatrienal (16.8-19.2 ml effluent). The rate of hydroperoxide breakdown was estimated by plotting the integrated radioactivity associated with the
peak of unconverted hydroperoxide versus time. When
2-hydroperoxylinolenic acid was allowed to degrade in the presence of
enzyme preparations, a portion of the product consisted of
2-hydroxylinolenic acid and nor-linolenic acid. These compounds are
expected to elute as their salts together with the hydroperoxide,
however, because of the small and variable amounts of these
decomposition products (together 10% or less), no attempt was made to
correct for their presence. In method B,
2(R,S)-hydroperoxyoleic acid (30 µM) was stirred with the test preparation (6 ml) at 23 °C. Aliquots of 1 ml
were removed at different times and added to 5 ml of ethanol containing
25 mg of stannous chloride. After 20 min at 23 °C, an internal
standard of tetracosanoic acid (70 nmol) was added and the mixtures
were extracted with diethyl ether. Aliquots of the methyl-esterified
product was subjected to GLC (column temperature, 270 °C) and the
peak areas of methyl 2-hydroxyoleate (retention time, 3.6 min) formed
by reduction of 2-hydroperoxyoleic acid remaining in the incubation
mixture, and of methyl tetracosanoate (retention time, 7.8 min) due to
the added internal standard were determined. The rate of hydroperoxide
breakdown was calculated from plots of the ratio between the peak areas
of methyl 2-hydroxyoleate and methyl tetracosanoate versus
time. As with method A, no attempt was made to correct for
the small amount of 2-hydroxy acid produced from the hydroperoxide
during the incubation period. In some experiments, the reduced samples
containing methyl 2-hydroxyoleate were derivatized with
()-menthoxycarbonyl chloride, purified by TLC, and subjected to GC-MS
operated in the selected ion monitoring mode using the ions
m/z 294 and 262. By combining the peak areas of the MC
derivatives of methyl 2(S)-hydroxyoleate (retention
time, 13.15 min) and methyl 2(R)-hydroxyoleate (13.37 min)
with the half-life data, it was possible to separately monitor
breakdown of the "R" and "S" enantiomers of 2-hydroperoxyoleate.
Chemical Methods--
Configurational determination of 2-hydroxy
acids were performed by analysis of MC derivatives by GLC or GC-MS
(30). MO derivatives of carbonyl compounds and Me3Si ethers
of hydroxy compounds were prepared as described previously (31).
[2H9]Me3Si derivatives,
occasionally needed to verify correct interpretation of mass spectra,
were prepared by derivatization with
[2H18]N,O-bis(trimethylsilyl)acetamide
(98%, Cambridge Isotope Laboratories, Andover, MA) at 23 °C for 30 min. For analysis of 2-hydroperoxy acids by GC-MS, the hydroperoxides
(10-50 µg) were derivatized with BSTFA (0.1 ml) and an aliquot of
1-2 µl containing the Me3Si peroxide/Me3Si
ester was directly injected onto the column. Hydroperoxides were
reduced into alcohols by treatment with SnCl2 in ethanol (5 mg/ml) at room temperature for 10 min, or with triphenyl phosphine in
diethyl ether (10 mg/ml) at room temperature for 1 h. Catalytic hydrogenation was performed with platinum catalyst (3 mg) and methanol
(1 ml) as the solvent. Oxidative ozonolysis was carried out as
described (30) using an ozone generator model T-12 purchased from TriO3
Industries, Fort Pierce, FL. Incubations under 18O gas were
conducted in an all-glass apparatus attached to a high vacuum line.
18O2 (isotopic purity, 96%) was obtained from
Larodan AB, Malmö, Sweden.
Chromatographic and Instrumental Methods--
RP-radio-HPLC was
performed with columns of Nucleosil 100-5 C18 (250 × 4.6 mm) purchased from Macherey-Nagel (Düren, Germany). The
solvent systems consisted of mixtures of acetonitrile, water, 2 M hydrochloric acid in volume proportions 55:45:0.013
(system I), 60:40:0.013 (system II), 65:35:0.013 (system III), or
80:20:0.013 (system IV). The absorbance (210 nm) and radioactivity of
HPLC effluents were determined on-line using a Spectromonitor III
ultraviolet detector (Laboratory Data Control, Riviera Beach, FL) and a
liquid scintillation counter (IN/US Systems, Tampa, FL), respectively. GLC was performed with a Hewlett-Packard (Avondale, PA) model 5890 gas
chromatograph equipped with a methylsilicone capillary column (length,
25 m; film thickness, 0.33 µm) and a flame ionization detector.
Helium at a flow rate of 25 cm/s was used as the carrier gas. Retention
times found on GLC were converted into C-values as described (31).
GC-MS was carried out with a Hewlett-Packard model 5970B mass selective
detector connected to a Hewlett-Packard model 5890 gas chromatograph
fitted with a 5% phenylmethylsilicone capillary column (length,
12 m; film thickness, 0.33 µm). In most runs the initial column
temperature was 120 °C and raised at 10 °C/min until 240 °C.
Ultraviolet spectra were recorded with a Hitachi (Tokyo, Japan) model
U-2000 UV/VIS spectrophotometer. Infrared spectrometry was carried out
on films using a Perkin-Elmer (Norwalk, CT) model 1650 Fourier
transform-infrared spectrophotometer. Radioactivity was determined with
a Packard Tri-Carb model 4450 liquid scintillation counter (Packard
Instruments, Downer's Grove, IL).
| |
RESULTS |
Oxygenation of Fatty Acids by Recombinant Oxygenases
Incubation of Linolenic Acid with Recombinant Enzymes from Tobacco
Leaves or Arabidopsis--
A preparation of the tobacco leaf oxygenase
obtained from insect cells infected with baculovirus carrying
pFASTBAC-tob.A5.2 was stirred for 20 min at 23 °C with 100 µM
[9,10,12,13,15,16-3H6]linolenic acid. The
product isolated by extraction with diethyl ether (recovery of
radioactivity, 87%) was analyzed by RP-radio-HPLC. Three peaks of
radioactive compounds appeared in addition to the peak of linolenic
acid remaining unconverted (Fig.
1A). Compounds 1 (7% of the
recovered product, 22.9 ml effluent), 2 (1%, 38.4 ml effluent), and 3 (29%, 85.8 ml effluent) were collected for structural determination.
As seen in Fig. 1B, a corresponding incubation using cells
infected with virus carrying the pFASTBAC vector only gave undetectable
conversion of the added tritium-labeled linolenic acid. Incubation of
preparations from cells infected with virus carrying
pFASTBAC-ara.N38086 (Arabidopsis oxygenase) gave rise to the
same products as those formed by the tobacco leaf enzyme,
i.e. compound 1 (4%), compound 2 (1%), and compound 3 (34%) (Fig. 2A). As seen in
Fig. 2B, the same products, and an additional one (compound
4) eluting just after compound 1, were produced upon incubation of
linolenic acid with a preparation of cucumber (see below).
View larger version (10K):
[in this window]
[in a new window]
|
Fig. 1.
Reversed phase HPLC radiochromatograms of
products formed from linolenic acid incubated with preparations from
insect cells. Panel A,
[9,10,12,13,15,16-3H6]linolenic acid (100 µM) was stirred with a preparation of cells expressing
the tobacco leaf oxygenase in potassium phosphate buffer, pH 6.7 (5.5 ml; 2.4 mg of protein), at 23 °C for 20 min and the product was
isolated by extraction with diethyl ether. Panel B, same as
A but using a preparation of control cells not expressing
oxygenase. Solvent system II at a flow rate of 1.5 ml/min was used.
1, 2, 3, compounds 1-3; 18:3, linolenic
acid.
|
|
View larger version (13K):
[in this window]
[in a new window]
|
Fig. 2.
Reversed phase HPLC radiochromatograms of
products formed from linolenic acid incubated with a preparation from
insect cells or with a cucumber preparation. Panel A,
[9,10,12,13,15,16-3H6]linolenic acid (100 µM) was stirred with a preparation of the
Arabidopsis oxygenase in potassium phosphate buffer, pH 6.7 (10 ml, 1.1 mg of protein), at 23 °C for 20 min and the product was
isolated by extraction with diethyl ether. Panel B,
[9,10,12,13,15,16-3H6]linolenic acid (268 µM) was stirred with whole homogenate of cucumber at
23 °C for 20 min and the isolated product was analyzed by HPLC.
Solvent system II at a flow rate of 1.5 ml/min was used. 1, 2, 3, 4, compounds 1-4; 18:3, linolenic acid.
|
|
Identification of Compound 1--
The UV spectrum of compound 1 was featureless, indicating the absence of conjugated double bonds. On
RP-HPLC, compound 1 co-chromatographed with authentic
2-hydroxylinolenic acid. Considerable chromatographic tailing was
observed for both compounds. The retention time found on GLC (C-value,
18.96) and the mass spectrum of the methyl ester of compound 1, were
identical to those of methyl 2-hydroxylinolenate (see "Experimental
Procedures"). Results obtained upon GC-MS analysis of the
Me3Si derivatives of the methyl esters of compound 1 and 2-hydroxylinolenic acid were identical. Catalytic hydrogenation of
compound 1 followed by esterification produced methyl
2-hydroxystearate. Analysis by GLC of the MC derivative of the
methyl ester of compound 1 showed that the absolute configuration at
C-2 was R (less than 1% of the S enantiomer).
Degradation of the MC derivative of the methyl ester of compound 1 by
oxidative ozonolysis produced the MC derivative of methyl hydrogen
2(R)-hydroxyazelate, thus confirming the R
configuration at C-2 as well as the presence of a double bond in the
9 position. Based on these results, compound 1 was
identified as 2(R)-hydroxy-9(Z),12(Z),15(Z)-octadecatrienoic
acid (2(R)-hydroxylinolenic acid) (Fig.
3).
Identification of Compound 2--
Compound 2 co-chromatographed
with authentic
8(Z),11(Z),14(Z)-heptadecatrienoic
acid on RP-HPLC. Furthermore, the retention time found on GLC (C-value,
16.76) and the mass spectrum of the methyl ester were identical to
those of methyl
8(Z),11(Z),14(Z)-heptadecatrienoate. Catalytic hydrogenation of compound 2 followed by
methyl-esterification afforded methyl heptadecanoate, whereas
oxidative ozonolysis of compound 2 yielded suberic acid as the
main non-volatile fragment. On the basis of these results, compound 2 was identified as
8(Z),11(Z),14(Z)-heptadecatrienoic acid (nor-linolenic acid) (Fig. 3).
Identification of Compound 3--
Compound 3 co-chromatographed
with authentic
8(Z),11(Z),14(Z)-heptadecatrienal on
RP-HPLC. Both compounds gave an unusually broad but symmetric peak
(cf. Figs. 1 and 2). The C-value found on GLC (15.78) and
the mass spectrum were identical to those of 8(Z),11(Z),14(Z)-heptadecatrienal.
Furthermore, the MO derivatives of compound 3 and the authentic
reference had identical C-values and mass spectra. Reduction of
compound 3 with NaBH4 afforded 8(Z),11(Z),14(Z)-heptadecatrienol, the
Me3Si derivative of which gave a mass spectrum showing
prominent ions at m/z 322 (M+; 3), 307 (M+ 15; loss of ·CH3; 2), 266 (3),
183 (4), 135 (11), 108 (54), 79 (99), and 75 (100). Catalytic
hydrogenation of reduced compound 3 afforded 1-heptadecanol. Based on
these results, compound 3 was identified as
8(Z),11(Z),14(Z)-heptadecatrienal
(Fig. 3).
Products formed from Linoleic Acid--
Preparations of the
tobacco leaf and Arabidopsis enzymes (2 and 0.5 mg of
protein, respectively) in 5 ml of potassium phosphate buffer, pH 7.4, were stirred at 23 °C for 30 min with 70 µM linoleic acid. The product was treated with diazomethane and analyzed by GLC and
GC-MS. Apart from methyl linoleate (C-17.69) corresponding to unreacted
linoleic acid, three peaks appeared having the following C-values:
C-15.73, C-16.71, and C-18.96. The mass spectrum recorded on the first
mentioned peak showed prominent ions at m/z 250 (M+; 4%), 221 (1), 207 (1), 193 (1), 179 (1), 151 (3), 95 (36), 81 (62), 67 (100), and 55 (61), thus indicating a C17 diunsaturated aldehyde. Treatment with O-methylhydroxylamine
afforded two peaks due to the syn/anti isomers of the
aldehyde, the mass spectra of which showed prominent ions at
m/z 279 (M+; 1%), 264 (M+ 15;
loss of ·CH3; 1), 248 (M+ 31; loss of
·OCH3; 57); 180 (11), 168 (7), 95 (30), 81 (57), 67 (100), and 55 (78). The second peak was due to methyl nor-linoleate as judged by its C-value (16.71) and its mass spectrum, which showed prominent ions at m/z 280 (M+; 12%), 249 (M+ 31; loss of ·OCH3; 7), 206 (4),
150 (16), 95 (52), 81 (81), 67 (100), and 55 (75). The last peak
(C-18.96) provided a mass spectrum showing a molecular ion at
m/z 310 in agreement with a 2-hydroxyoctadecadienoate methyl
ester. A more informative spectrum was recorded on the Me3Si derivative, i.e. m/z 382 (M+; 2%), 367 (M+ 15; loss of
·CH3; 20), 323 (M+ 59; loss of
·COOCH3; 18), 306 (3), 233 (4), 161 (Me3SiO+ = CH-COOCH3; 4), 159 (14),
129 (Me3SiO+ = CH-CH = CH2;
14), 89 (Me3SiO+; 43), and 73 (Me3Si+; 100). On the basis of these data, the
linoleic acid-derived compounds were identified as
8(Z),11,(Z)-heptadecadienal,
8(Z),11(Z)-heptadecadienoic acid, and
2-hydroxy-9(Z),12(Z)-octadecadienoic acid (Table
I). The same set of compounds was
produced from linoleic acid (100 µM) upon incubation with
a whole homogenate preparation of cucumber.
View this table:
[in this window]
[in a new window]
|
Table I
Products isolated following incubation of fatty acids with
recombinant oxygenases from tobacco leaves or Arabidopsis or with
homogenate of cucumber
|
|
Products Formed from Oleic Acid--
Incubation of 70 µM oleic acid with the tobacco leaf or
Arabidopsis enzyme preparations carried out as described for
linoleic acid provided three compounds which were identified by their
C-values and mass spectra as 8(Z)-heptadecenal,
8(Z)-heptadecenoic acid, and
2-hydroxy-9(Z)-octadecenoic acid (Table I). The mass
spectrum of the aldehyde showed a molecular ion at m/z 252, which was shifted to m/z 281 upon treatment with
O-methylhydroxylamine. The methyl ester of the 2-hydroxy
acid produced the expected molecular ion at m/z 312 (4%)
and a prominent ion at m/z 253 (24%) formed by elimination of the carbomethoxy group. Incubation of oleic acid (100 µM) with the cucumber preparation resulted in the
formation of an identical set of products.
Products Formed from Palmitic Acid--
Palmitic acid (70 µM) incubated with the tobacco leaf,
Arabidopsis, or cucumber enzyme preparations produced three
compounds which were identified as pentadecanal, pentadecanoic acid,
and 2-hydroxypalmitic acid. The two first mentioned compounds gave C-values and mass spectra which were identical to those of the authentic compounds, and the 2-hydroxy acid gave identical data as
those of the 2-hydroxy acid formed upon stannous chloride reduction of
2-hydroperoxypalmitic acid.
Kinetic Constants of Recombinant Oxygenases--
Fatty acids were
stirred with preparations of the tobacco leaf and
Arabidopsis enzymes (protein, 0.13 and 0.07 mg/ml,
respectively) at 30 °C in 1.5 ml of 0.1 M Tris buffer,
pH 8.0, and the rate of oxygen uptake was monitored using a Clark
oxygen electrode. The Km and
Vmax values were determined from
double-reciprocal plots of the maximum velocity of oxygen uptake and
substrate concentration. The results are given in Table
II. As seen, linolenic, linoleic, and
oleic acids were all good substrates for the two enzymes and had
Km values of 1-2 µM (tobacco leaf
oxygenase) and 13-18 µM (Arabidopsis
oxygenase). In agreement with previous results (22), arachidonic acid
was a less effective substrate compared with the 18-carbon fatty
acids.
View this table:
[in this window]
[in a new window]
|
Table II
Kinetic constants of recombinant oxygenases
Consumption of O2 by protein extracts containing recombinant
oxygenases from tobacco (pFASTBAC-tob.A5.2) or Arabidopsis
(pFASTBAC-ara.N38086) was evaluated after incubation with increasing
concentrations of various fatty acids in 0.1 M Tris buffer,
pH 8.0, at 30 °C. Kinetic constants were estimated from
Lineweaver-Burk plots.
|
|
Biosynthesis of 2(R)-Hydroperoxylinolenic Acid
Formation of 2(R)-Hydroperoxylinolenic Acid by Recombinant
Enzymes--
Arabidopsis enzyme in 0.1 M
potassium phosphate buffer, pH 7.4 (5 ml; protein, 0.2 mg/ml), was
stirred at 0 °C for 20 min with 50 µM [9, 10, 12,13,15,16-3H6]linolenic acid. The product
was rapidly extracted with diethyl ether and subjected to
RP-radio-HPLC. As seen in Fig. 4, in
addition to compounds 1-3 (3, 2, and 8%, respectively, of the
recovered radioactivity), an additional peak of radioactivity appeared
immediately after compound 1. This material, i.e. compound 4 (24% of the recovered radioactivity), was converted into compound 1 (2-hydroxylinolenic acid) upon treatment with mild reducing agents such
as SnCl2 or triphenylphosphine, suggesting that it was due
to the 2-hydroperoxy derivative of linolenic acid. Reduction of
compound 4 with sodium borodeuteride led to the formation of
2-hydroxylinolenic acid with no detectable incorporation of deuterium,
thus excluding the presence of a keto function. Analysis of compound 4 by GC-MS without derivatization resulted in thermally induced
decarboxylation and the appearance of a single peak giving the same
mass spectrum as
8(Z),11(Z),14(Z)-heptadecatrienal. A
similar analysis carried out following trimethylsilylation using BSTFA
reagent showed peaks due to
8(Z),11(Z),14(Z)-heptadecatrienal (6.4 min retention time, 23%), the Me3Si ester of
2-ketolinolenate (10.3 min, 12%), the Me3Si ether/ester of
2-hydroxylinolenate (10.8 min, 17%), the Me3Si ether/ester
of the enol form of 2-ketolinolenate (11.0 min, 13%), and the
Me3Si peroxide/ester of 2-hydroperoxylinolenate (11.5 min,
35%). This profile of products was analogous to that observed for the
Me3Si derivative of 2-hydroperoxyoleate (see "Experimental Procedures"). The mass spectrum of the derivative of
2-hydroperoxylinolenate showed prominent ions at m/z 439 (M+ 15; loss of ·CH3; 2%), 422 (M+ 32; rearrangement with loss of CH3OH;
12), 337 (M+ 117; loss of ·COOSiMe3;
2), 247 (337-90; 8), 163 (Me3Si-O-O+ = SiMe2; 18), 147 (Me3Si-O+ = SiMe2; 39), 89 (Me3SiO+; 52), and
73 (Me3Si+; 100) (Fig.
5A). This fragmentation was
analogous to that observed for the Me3Si derivative of
2-hydroperoxyoleate. In another experiment, the Arabidopsis
enzyme was incubated with linolenic acid under an atmosphere of
18O2. An aliquot of compound 4 isolated by
RP-HPLC was treated with BSTFA and subjected to GC-MS analysis.
Analysis of the isotope composition using the ions formed by
elimination of ·CH3 (m/z 439, 441, and
443) showed the presence of molecules containing 2 atoms of
18O (78%), 1 of 18O (4%), and no
18O (18%). Although the extent of 18O labeling
was not complete, it was clear that compound 4 was formed from
linolenic acid by incorporation of one molecule of dioxygen, as would
be expected for a hydroperoxide. The mass spectrum of the
Me3Si derivative of 18O2-labeled
compound 4 showed the expected shifts compared with the spectrum of the
unlabeled derivative, i.e. (number of 18O in
parentheses): 443 (2), 424 (1), 341 (2), 249 (1), 165 (1), 149 (1), 147 (0), 91 (1), 73 (0) (Fig. 5B). On the basis of the data
described, compound 4 was identified as
2-hydroperoxy-9(Z),12(Z),15(Z)-octadecatrienoic
acid (2-hydroperoxylinolenic acid). The absolute configuration at C-2
was R as shown by GLC analysis of the MC derivative of
2-hydroxylinolenic acid prepared by reduction with
SnCl2.
View larger version (10K):
[in this window]
[in a new window]
|
Fig. 4.
Reversed phase HPLC radiochromatogram of
product formed from linolenic acid incubated with a preparation from
insect cells at 0 °C.
[9,10,12,13,15,16-3H6]Linolenic acid (50 µM) was stirred with a preparation of cells expressing
the Arabidopsis oxygenase at 0 °C for 20 min and the
product was isolated by extraction with diethyl ether. Solvent system I
(0-25 min) followed by system IV (25-40 min) at a flow rate of 1.8 ml/min was used. 1, 2, 3, 4, compounds 1-4;
18:3, linolenic acid. The peak of UV absorption due to BHT
present in the diethyl ether used has been substracted.
|
|
View larger version (18K):
[in this window]
[in a new window]
|
Fig. 5.
Mass spectra of derivatives of
2-hydroperoxylinolenic acid. Panel A, mass spectrum of
bis(trimethylsilyl) derivative of 2-hydroperoxylinolenic acid.
Panel B, mass spectrum of bis(trimethylsilyl) derivative of
[2-18O2]2-hydroperoxylinolenic acid.
|
|
Incubation of Linolenic Acid with Enzyme Preparations from
Cucumber--
[9,10,12,13,15,16-3H6]Linolenic
acid (268 µM) was stirred with whole homogenate of
cucumber at 23 °C for 20 min and the product isolated by extraction
with diethyl ether (recovery of radioactivity, 74%) was analyzed by
RP-radio-HPLC. As seen in Fig. 2B, the main products formed
from the labeled linolenic acid were compound 1 (10% of the recovered
radioactivity), compound 2 (3%), compound 3 (18%), and compound 4 (8%). Compounds 1-4 were identified as described above and found to
be 2(R)-hydroxylinolenic acid,
8(Z),11(Z),14(Z)-heptadecatrienoic acid,
8(Z),11(Z),14(Z)-heptadecatrienal, and
2(R)-hydroperoxylinolenic acid, respectively. The
radioactive materials eluting before compound 1, and the materials
eluting between compounds 4 and 2, were lipoxygenase products as judged
by the finding that lipoxygenase inhibitors blocked their formation.
The fraction sedimenting at 48,000 × g of homogenate
of cucumber was a convenient source of dioxygenase activity. By
incubating linolenic acid with this fraction at 0 °C (see Fig.
6 and "Eperimental Procedures") it
was possible to prepare milligram amounts of
2(R)-hydroperoxylinolenic acid.
View larger version (12K):
[in this window]
[in a new window]
|
Fig. 6.
Reversed phase HPLC radiochromatogram
of product formed from linolenic acid incubated with a cucumber
preparation at 0 °C.
[9,10,12,13,15,16-3H6]Linolenic acid (152 µM) was stirred with the 48,000 × g
particle fraction of homogenate of cucumber at 0 °C for 30 min and
the product was isolated by extraction with diethyl ether. Solvent
system I (0-25 min) followed by system III (25-55 min) at a flow rate
of 2 ml/min was used. 1, 2, 3, 4, compounds 1-4;
18:3, linolenic acid. The peak of UV absorption due to BHT
present in the diethyl ether used has been substracted.
|
|
Conversions of 2-Hydroperoxy Fatty Acids
Degradation of 2(R)-Hydroperoxylinolenic Acid in
Buffer--
Tritium-labeled 2(R)-hydroperoxylinolenic acid
(35 µM) was added to 0.1 M potassium
phosphate buffer, pH 7.4, and kept at 23 °C for 30 min. The product
was analyzed by RP-radio-HPLC and found to consist of unchanged
hydroperoxide (48%),
8(Z),11(Z),14(Z)-heptadecatrienal (46%), and
8(Z),11(Z),14(Z)-heptadecatrienoic
acid (6%). Longer times of treatment led to further loss of
hydroperoxide with concomitantly increased formation of
heptadecatrienal and heptadecatrienoic acid. An increased ratio of
heptadecatrienoic acid/heptadecatrienal was observed with longer times
of treatment, indicating that the heptadecatrienoic acid was formed
from the aldehyde by air oxidation. Analysis of hydroperoxide
degradation using method A demonstrated a first order decay
with a rate constant of 0.0234 min1 corresponding to a
half-life time of 30 min. 2-Hydroxylinolenic acid was not detectable in
these experiments.
Degradation of 2(R)-Hydroperoxylinolenic Acid in Enzyme
Preparations--
Tritium-labeled 2(R)-hydroperoxylinolenic
acid (25 µM) was added to preparations of cells
expressing the tobacco leaf or Arabidopsis enzymes, or none
of these enzymes, and kept at 23 °C for 20 min. Analysis by
RP-radio-HPLC showed that only trace amounts of hydroperoxide remained.
The product compositions were similar in the three incubations and
consisted of
8(Z),11(Z),14(Z)-heptadecatrienal
(about 90%), 2-hydroxy-9(Z),12(Z),15(Z)-octadecatrienoic
acid (about 7%), and 8(Z),11(Z),14(Z)-heptadecatrienoic
acid (about 3%). Degradation of the hydroperoxide followed first-order
kinetics with k = 0.221-0.245 min1
corresponding to half-life times ranging from 2.8 to 3.1 min. No
significant difference in the rates of degradation of
hydroperoxide in the presence of tobacco leaf or Arabidopsis
enzymes or in their absence was noticeable (Fig.
7).
View larger version (13K):
[in this window]
[in a new window]
|
Fig. 7.
Rates of degradation of
2(R)-hydroperoxylinolenic acid in the presence of
preparations from insect cells.
[9,10,12,13,15,16-3H6]2(R)-Hydroperoxylinolenic
acid (35 µM) was stirred with preparations from cells
(0.8 ml) for 1-10 min at 23 °C. The amounts of remaining
hydroperoxide were determined by HPLC (method A).  ,
preparation from cells lacking recombinant oxygenases;  , preparation
from cells expressing recombinant oxygenase from tobacco leaves;  ,
preparation from cells expressing oxygenase from
Arabidopsis.
|
|
Degradation of 2(R,S)-Hydroperoxyoleic Acid in Enzyme
Preparations--
Tritium-labeled 2(R,S)-hydroperoxyoleic
acid (30 µM) was stirred at 23 °C with preparations of
recombinant oxygenases or with the 48,000 × g particle
fraction of homogenate of cucumber. Analysis by RP-radio-HPLC
demonstrated a rapid degradation of the hydroperoxide with concomitant
formation of 8(Z)-heptadecenal,
2-hydroxy-9(Z)-octadecenoic acid, and
8(Z)-heptadecenoic acid. The rate of hydroperoxide
degradation as determined by method B followed first-order
kinetics with half-life times of 5.9 min (cucumber preparation) or
2.4-2.7 min (preparations of insect cells expressing the tobacco leaf
or Arabidopsis enzymes). In order to determine whether
degradation of the hydroperoxide was associated with chiral
discrimination, samples removed at the different time points were
derivatized with ()-menthoxycarbonyl chloride and subjected to steric
analysis. As shown in Fig. 8, no
significant difference in the rates of degradation of the
2(R)- and 2(S)-enantiomers of the hydroperoxide
was noticeable (half-life times for 2(R)- and
2(S)-enantiomers in the presence of tobacco leaf enzyme, 2.7 and 2.5 min, respectively; half-life times for 2(R)- and
2(S)-enantiomers in the presence of Arabidopsis
enzyme, 2.4 and 2.5 min, respectively). Similar results were obtained in incubations with preparations of cells not expressing
oxygenases.
View larger version (12K):
[in this window]
[in a new window]
|
Fig. 8.
Rates of degradation of individual
enantiomers of 2(R,S)-hydroperoxyoleic acid in the
presence of enzyme preparations.
[9,10-3H2]2(R,S)-Hydroperoxyoleic
acid (30 µM) was added to enzyme preparations (6.5 ml)
and kept at 23 °C. Aliquots (1.2 ml) were removed during the time
interval 1-10 min and added to ethanol containing stannous chloride.
Amounts of 2-hydroxyoleate, reflecting residual 2-hydroperoxyoleate,
were determined by GLC (method B). Samples were derivatized
with ()-menthoxycarbonyl chloride and the enantiomeric composition of
2-hydroxyoleate at the different time points was determined by GC-MS.
A, incubation with tobacco leaf oxygenase; B,
incubation with Arabidopsis oxygenase. ,
2(R,S)-hydroperoxyoleate; ,
2(R)-hydroperoxyoleate; ,
2(S)-hydroperoxyoleate.
|
|
2(R)-Hydroperoxylinolenic Acid as a Substrate for
Peroxygenase--
A particulate fraction from homogenate of V. faba seeds containing peroxygenase (6) was suspended in buffer
(0.5 ml; 0.3 mg of protein). The preparation was stirred with
5,8,11,14-eicosatetraynoic acid (50 µM) at 23 °C for 5 min in order to block lipoxygenase activity and subsequently treated
with [9,10-3H2]oleic acid (100 µM) and 2-hydroperoxylinolenic acid at 23 °C for 15 min. Control incubations performed in the absence of
2-hydroperoxylinolenic acid, or in the presence of
9(S)-HPOD, were also performed. Conversion of the
tritium-labeled oleic acid into cis-9,10-epoxyoctadecanoic acid (6) was monitored by RP-radio-HPLC. As seen in Fig.
9, 2-hydroperoxylinolenic acid supported
epoxidation of oleic acid into 9,10-epoxyoctadecanoic acid. In contrast
to epoxidations carried out with 9(S)-HPOD and other
lipoxygenase-generated hydroperoxides, the 2-hydroperoxylinolenic
acid-supported epoxidation appeared to plateau at a hydroperoxide
concentration of about 100 µM. Whether this phenomenon
was due to enhanced rate of inactivation of peroxygenase (cf. Ref. 32) by the 2-hydroperoxylinolenic acid remains to be determined. The absolute configuration of the
cis-9,10-epoxyoctadecanoic acid produced from oleic acid in
the presence of peroxygenase and 2-hydroperoxylinolenic acid was
determined (33) and found to be 9(R),10(S) (81%)
and 9(S),10(R) (19%). This result was similar to
that earlier found with other hydroperoxides, strengthening the notion
that the stereochemistry of peroxygenase-catalyzed epoxidation is
solely dictated by the enzyme and is not related to the stereochemistry
of the hydroperoxide co-substrate (6, 32). In another experiment,
2-hydroperoxyoleic acid (17 µM) was incubated with the
peroxygenase preparation in the absence of oxidizable co-substrate. The
product was methyl-esterified and subjected to TLC using a solvent
system of ethyl acetate:hexane, 20:80 (v/v). Two bands appeared, the
less polar of which (RF = 0.59) was due to methyl
2-hydroxy-9(Z)-octadecenoate as judged by GC-MS analysis.
The more polar material (RF = 0.32) was analyzed as
its Me3Si derivative by GC-MS. Prominent ions were observed
at m/z 369 (M+ 31; loss of
·OCH3; 28), 341 (M+ 59; loss of
·COOCH3; 15), 325 (34), 251 (341-90; 4), 199 (12),
159 (18), 129 (Me3SiO+ = CH-CH = CH2; 18), and 73 (Me3Si+; 100).
Treatment of the material with perchloric acid in aqueous tetrahydrofuran afforded methyl 2,9,10-trihydroxyoctadecanoate, thus
confirming the identity of the compound produced from
2-hydroperoxyoleic acid in the presence of peroxygenase as
9,10-epoxy-2-hydroxyoctadecanoic acid.
View larger version (14K):
[in this window]
[in a new window]
|
Fig. 9.
Peroxygenase-catalyzed epoxidations of oleic
acid. Suspensions of the 105,000 × g particle
fraction of homogenate of V. faba (0.5 ml) were stirred with
50 µM 5,8,11,14-eicosatetraynoic acid at 23 °C for 5 min and subsequently treated with 100 µM tritium-labeled
oleic acid and hydroperoxide at 23 °C for 15 min. Formation of
tritium-labeled 9,10-epoxyoctadecanoic acid was monitored by
RP-radio-HPLC. , incubations with
2(R)-hydroperoxylinolenic acid; , incubations with
9(S)-HPOD.
|
|
| |
DISCUSSION |
A pathogen-inducible oxygenase (PIOX) in tobacco leaves and a
homologous enzyme from Arabidopsis were identified in recent work (22). Sequence and functional analysis of the piox
cDNA-encoded protein showed significant homology with
prostaglandin-endoperoxide H synthase types-1 and -2, key enzymes in
the synthesis of lipid signal molecules in vertebrates. Endoperoxide
synthases are dual function enzymes possessing cyclooxygenase and
peroxidase activities (34). The recombinant PIOX proteins from tobacco
and Arabidopsis possessed oxygenase activity toward several
polyunsaturated fatty acids, however, peroxidase activity could not be
demonstrated (22).
In order to establish the catalytic function of the oxygenase from
tobacco leaves and its homologue from Arabidopsis,
incubations with linolenic acid were performed and the isolated
products were characterized by chemical and spectral methods. With both
enzymes, the major compound consisted of a C17 unsaturated
aldehyde, which was identified as
8(Z),11(Z),14(Z)-heptadecatrienal
by comparison with authentic material. In addition, small amounts of
2(R)-hydroxylinolenic acid and the C17 homologue
of linolenic acid, i.e.
8(Z),11(Z),14(Z)-heptadecatrienoic acid, were produced. Other fatty acids, including linoleic, oleic, and
palmitic acids, were metabolized in an analogous way (Tables I and II).
The product profile observed, consisting of a chain-shortened aldehyde,
a 2-hydroxy acid, and a chain-shortened fatty acid, was the same as the
profile encountered previously in studies of -oxidation in plant
tissues. This metabolic pathway was characterized by Stumpf (35), who
found that a preparation from peanut cotelydons catalyzed the oxidation
of palmitic acid into a long chain fatty aldehyde with concomitant
liberation of CO2. In subsequent work, -oxidation of
various Cn fatty acids into Cn-1 aldehydes
together with varying amounts of Cn-hydroxy acids and
Cn-1 fatty acids has been studied in preparations of pea leaves (36), cucumber (27-29), potato (37), and the green alga
Ulva pertusa (38). The -oxidation enzymes have been suggested to operate together with aldehyde dehydrogenase and NAD+ and thus to provide a pathway for stepwise degradation
of fatty acids into shorter chain homologues (for review, see Ref.
39).
When the recombinant enzymes from tobacco and Arabidopsis
were incubated with substrate at 0 °C rather than at room
temperature, formation of aldehyde was suppressed and a new main
product was formed, i.e. compound 4 (Fig. 4). Compound 4 was
converted into 2(R)-hydroxylinolenic acid upon treatment
with mild chemical reductants and underwent thermal decarboxylation
into
8(Z),11(Z),14(Z)-heptadecatrienal. These results indicated that compound 4 was identical to
2(R)-hydroperoxylinolenic acid, a new member of the oxylipin
family of compounds. The trimethylsilyl peroxide/ester derivative of
2-hydroperoxylinolenic acid was sufficiently stable to be analyzed by
gas chromatography-mass spectrometry (Fig. 5A;
cf. Refs. 40 and 41). As expected, an incubation carried out
under 18O gas resulted in incorporation of
18O2 and formation of doubly
18O-labeled hydroperoxide (Fig. 5B). Isolation
of 2(R)-hydroperoxylinolenic as the main product of
oxygenation of linolenic acid defined the tobacco and
Arabidopsis enzymes as fatty acid -dioxygenases (Fig. 10). The product profile observed
following incubation of linolenic acid with the well studied
-oxidation system in cucumber (27-29) (Figs. 2B and 6)
was similar to that observed in the corresponding incubations with the
recombinant -dioxygenases (Figs. 1A, 2A, and
4), thus suggesting the general involvement of -dioxygenase in plant
-oxidation.
View larger version (23K):
[in this window]
[in a new window]
|
Fig. 10.
Enzymatic formation of
2(R)-hydroperoxylinolenic acid and its further
conversions. S and SO, substrate and
oxidized substrate, respectively, in the peroxygenase-catalyzed
reaction.
|
|
Isolation and characterization of 2(R)-hydroperoxylinolenic
acid was of interest in relation to the mechanism of -oxidation. Already in 1974, Shine and Stumpf (42) found that inclusion of
glutathione and glutathione peroxidase to incubations of palmitic acid
with systems for -oxidation resulted in increased formation of
2-hydroxypalmitic acid and a concomitant decrease in the formation of
aldehyde and CO2. On the basis of this result, a
2-hydroperoxide was proposed as an intermediate in -oxidation (42).
This hypothesis was recently supported by the finding that incubations
of fatty acids with a preparation from pea leaves carried out in the
presence of stannous chloride afforded enantiomerically pure
2(R)-hydroxy acids at the expense of aldehydes (43), and
very recently by the isolation of 2(R)-hydroperoxypalmitic
acid in incubations of palmitic acid with the -oxidation system from
the green alga U. pertusa (44).
2(R)-Hydroperoxylinolenic acid isolated in the present work
was considerably less stable than the lipoxygenase-type of fatty acid
hydroperoxides. The products formed upon nonenzymatic decomposition consisted of heptadecatrienal (about 90%) accompanied by small and
variable amounts of 2-hydroxylinolenic acid and heptadecatrienoic acid.
Methodology for estimation of the rate of breakdown of
2-hydroperoxylinolenic acid was devised. Chemical degradation of the
hydroperoxide in aqueous buffer, pH 7.4, at 23 °C followed
first-order kinetics with a half-life time of about 30 min. The rate of
decomposition was increased about 10-fold in the presence of
preparations of cells expressing the recombinant -dioxygenases. The
proximal and distal heme-binding histidines of
prostaglandin-endoperoxide H synthase-1 (His388 and
His207, respectively) as well as the distal glutamine
(Gln203) (34, 45) are conserved in the -dioxygenases
from tobacco and Arabidopsis (22), thus indicating that
these enzymes are heme proteins capable of further transformation of
fatty acid hydroperoxides. However, no specific hydroperoxide degrading
activity could be detected for the recombinant -dioxygenases, since
the increased rate of hydroperoxide degradation observed with
preparations of cells expressing -dioxygenases was observed also
with control cells not expressing -dioxygenase (Fig. 7).
Furthermore, degradation of a racemic hydroperoxide, i.e.
2(R,S)-hydroperoxyoleic acid, in the presence of
-dioxygenases proceeded in a non-stereoselective way (Fig. 8).
Although it is conceivable that -dioxygenases, when tested in
purified form (cf. Ref. 29), will promote degradation of
2-hydroperoxides, the available data suggest that other tissue-derived factors will prove more important in this respect.
The -oxidation pathway in mammals is of critical importance for
degradation of phytanic acid and other -methyl branched fatty acids
(46), however, the function of the corresponding pathway in plants is
not fully understood. The fact that PIOX, now established as a fatty
acid -dioxygenase involved in -oxidation, is pathogen-inducible,
suggests that the importance of the -oxidation pathway in plants may
be related to plant-pathogen interactions and defense reactions rather
than to serve as a pathway for stepwise degradation of fatty acids.
Possibly, the 2-hydroperoxides generated by action of -dioxygenases
can act as signaling compounds for inductions of genes and enzymes of
importance for plant's defense against pathogens (cf. Ref.
47). A direct toxic effect of the hydroperoxide or its degradation
products on the invading pathogen is also conceivable. Finally, because
2-hydroperoxides support peroxygenase-catalyzed epoxidation (Fig. 9),
biosynthesis of fungitoxic fatty acid epoxides (48) may take place by
coupling of the -dioxygenase and peroxygenase pathways.
| |
ACKNOWLEDGEMENTS |
The expert technical assistance of Gunvor
Hamberg and Tomas Cascon is gratefully acknowledged.
| |
FOOTNOTES |
*
This work was supported by Swedish Medical Research Council
Project number 03X-5170, by Vesical Co., Stockholm, Sweden, and the
Education and Science Ministry, Spain, Grant CICYT BIO97-0656.The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
To whom correspondence should be addressed: Dept. of Medical
Biochemistry and Biophysics, Div. of Physiological Chemistry II,
Karolinska Institutet, S-171 77 Stockholm, Sweden. Tel.:
46-8-728-7640; Fax: 46-8-736-0439; E-mail:
Mats.Hamberg@mbb.ki.se.
| |
ABBREVIATIONS |
The abbreviations used are:
PIOX, pathogen-inducible oxygenase;
BHT, 2,6-di-tert-butyl-4-methylphenol;
9(S)-HPOD, 9(S)-hydroperoxy-10(E),12(Z)-octadecadienoic
acid;
BSTFA, bis(trimethylsilyl)trifluoroacetamide;
GLC, gas-liquid
chromatography;
GC-MS, gas-liquid chromatography-mass spectrometry;
MC, ()-menthoxycarbonyl;
MO, O-methyloxime;
Me3Si, trimethylsilyl;
RP-HPLC, reversed phase high performance liquid
chromatography.
| |
REFERENCES |
| 1.
|
Hamberg, M.,
and Gardner, H. W.
(1992)
Biochim. Biophys. Acta
1165,
1-18[Medline]
[Order article via Infotrieve]
|
| 2.
|
Mueller, M. J.
(1997)
Physiol. Plant.
100,
653-663[CrossRef]
|
| 3.
|
Blée, E.
(1998)
Prog. Lipid Res.
37,
33-72[CrossRef][Medline]
[Order article via Infotrieve]
|
| 4.
|
Grechkin, A.
(1998)
Prog. Lipid Res.
37,
317-352[CrossRef][Medline]
[Order article via Infotrieve]
|
| 5.
|
Hamberg, M.,
Herman, C. A.,
and Herman, R. P.
(1986)
Biochim. Biopys. Acta
877,
447-457[Medline]
[Order article via Infotrieve]
|
| 6.
|
Hamberg, M.,
and Hamberg, G.
(1990)
Arch. Biochem. Biophys.
283,
409-416[CrossRef][Medline]
[Order article via Infotrieve]
|
| 7.
|
Blée, E.,
and Schuber, F.
(1990)
J. Biol. Chem.
265,
12887-12894 |
TOP
ABSTRACT
INTRODUCTION
