From the Département d'Enzymologie Cellulaire et Moléculaire, Institut de Biologie Moléculaire des Plantes, Centre National de la Recherche Scientifique UPR 406, 28 rue Goethe, 67000 Strasbourg, France
![]() |
ABSTRACT |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Several and in-chain fatty acid hydroxylases
have been characterized in higher plants. In microsomes from
Helianthus tuberosus tuber the
-2,
-3, and
-4
hydroxylation of lauric acid is catalyzed by one or a few closely
related aminopyrine- and MnCl2-inducible cytochrome
P450(s). To isolate the cDNA and determine the sequences of the(se)
enzyme(s), we used antibodies directed against a P450-enriched fraction
purified from Mn2+-induced tissues. Screening of a cDNA
expression library from aminopyrine-treated tubers led to the
identification of a cDNA (CYP81B1) corresponding to a
transcript induced by aminopyrine. CYP81B1 was expressed in yeast. A
systematic exploration of its function revealed that it specifically
catalyzes the hydroxylation of medium chain saturated fatty acids,
capric (C10:0), lauric (C12:0), and myristic (C14:0) acids. The same
metabolites were obtained with transgenic yeast and plant microsomes, a
mixture of
-1 to
-5 monohydroxylated products. The three fatty
acids were metabolized with high and similar efficiencies, the major position of attack depending on chain length. When lauric acid was the
substrate, turnover was 30.7 ± 1.4 min
1 and
Km(app) 788 ± 400 nM.
No metabolism of long chain fatty acids, aromatic molecules, or
herbicides was detected. This new fatty acid hydroxylase is typical
from higher plants and differs from those already isolated from other
living organisms.
![]() |
INTRODUCTION |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Engineering of lipid metabolism in oilseed crops has become one of the major objectives of plant biotechnology (1-4). Manipulation of fatty acid biosynthesis in transgenic plants offers a possibility for the improvement of the nutritional quality of vegetable oils, but also for redirecting plant metabolism toward production of renewable chemical feedstocks for industrial applications and replacement of petroleum-derived products. Alterations in fatty acid chain length, number, and position of double bonds have already been achieved. Next, valuable modifications will be achieved via introduction of functional groups to confer additional industrial commodities, such as increased or decreased solubility or fluidity, improved solvation of drugs or pesticides, presence of targets for chemical modifications, or synthesis of polymers. Among potential high value metabolites are the oxygenated (hydroxylated and epoxidized) products (5, 6).
Plants are able to synthetize a whole range of oxygenated fatty acids
(7). Some of them are major seed storage lipids in particular species.
For example, castor bean endosperm produces a seed oil containing up to
90% ricinoleic acid
(12R-hydroxyoctadec-cis-9-enoic acid). Other
hydroxylated and epoxidized fatty acids constitute the building units
of cutin and suberin, biopolymers that form the outer protective layers
of all plant species (8). Different types of oxygenated derivatives are
also released after mechanical stress or pathogen attack. Some of them
play an important role in the signaling pathways and act as triggers of
plant defense and plant development (9, 10). Others have been reported to have direct antimicrobial properties and to act as phytoalexins (11-14). Several classes of enzymes are involved in the formation of
oxygenated fatty acid metabolites, lipoxygenases, epoxygenases, and
desaturases, but the most versatile is the P450 superfamily of
monooxygenases. Data obtained with plant microsomes indicate that
several P450s catalyze fatty acid hydroxylation or epoxydation with
high regio- and stereospecificities (15). Attack of medium chain fatty
acids, capric (C10:0), lauric (C12:0), and myristic acids (C14:0), by
P450 enzymes occurs at different positions, depending on plant species.
Pea and other Leguminosae produce almost exclusively -hydroxylated
compounds (16, 17). Such
-hydroxylases are strongly and specifically
induced by clofibrate and other peroxisome proliferation-inducing
agents (18). In other plant species, attack of medium fatty acids
occurs in the chain. Microsomes from grass crops such as wheat and rice
generate principally
-1 and
-2 hydroxylated metabolites (19).
Lauric acid hydroxylation in wheat is induced in an additive manner by phenobarbital and the herbicide safener naphthalic anhydride, an
inducer of detoxifying enzymes used for selective protection of crops
against herbicide damage (20). A second type of in-chain metabolism was
first described in Helianthus tuberosus tuber (21-23), but
is also observed in several monocots like maize, tulip, or lily (17).
It results in the formation of
-2,
-3, and
-4 monohydroxylated
products. This type of fatty acid metabolism is strongly induced in
response to MnCl2, aminopyrine, and phenobarbital treatments of plant tissues (17, 22, 24). Parallel induction and
inhibition suggest that a single P450 catalyzes the
-2,
-3, and
-4 hydroxylations. High regioselectivity of attack of unsaturated analogues, on the other hand, would rather be indicative of the involvement of several and probably closely related enzymes (23, 25, 26).
A new strategy, based on the inducibility of such fatty acid in-chain fatty acid hydroxylases by multiple xenobiotics, has been devised to isolate their coding sequence(s) and to answer the question of their substrate and regiospecificities. We partially purified P450 proteins from MnCl2-induced H. tuberosus tuber tissues (27). Antibodies were raised against the partially purified protein fraction and used to screen a cDNA library from aminopyrine-treated tuber. This study reports the isolation of a cDNA corresponding to aminopyrine-induced transcript coding for a new P450 and the functional characterization of this P450 after expression in yeast. The protein is shown to catalyze the in-chain monohydroxylations of medium C10:0, C12:0, and C14:0 saturated fatty acids. A single P450 accounts for the formation of the different products found in plant microsomes. This new type of fatty acid hydroxylase has never been isolated from other living organisms.
![]() |
EXPERIMENTAL PROCEDURES |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Chemicals-- Aminopyrine was from Merck (Darmstadt, Germany). Benzoic acid, salicylic acid, coumarin, and 7-ethoxycoumarin were from Sigma (St. Quentin-Fallavier, France). Other coumarin derivatives were gifts from Dr. J. L. Rivière (Unité de Toxicologie Métabolique et Ecotoxicologie, Ecole Vétérinaire, Lyon, France). Phenoxazone derivatives were purchased from Pierce.
[3-trans-14C]Cinnamic acid was from Isotopchim (Ganagobie, France), [1-14C]lauric acid from CEA (Gif-sur-Yvette, France), and [1-14C]capric acid from Sigma (La Verpillière, France). [7-14C]Benzoic acid, [1-14C]myristic acid, [1-14C]palmitic acid, [1-14C]stearic acid, [1-14C]oleic acid, and [1-14C]linoleic acid were from DuPont (NEN, United Kingdom). [14C]Geraniol and S-[14C]naringenin were kindly provided by Dr. D. Hallahan (IACR-Roathamsted, Harpenden, UK) and Dr. G. Kochs (Institut für Biologie II, University of Freiburg, Germany), respectively. [dichlorophenyl-U-14C]Diclofop was kindly provided by Hoechst (Frankfurt am Main, Germany), [triazine-2-14C]chlorsulfuron by Du Pont de Nemours (Wilmington, Delaware), and [phenyl-U-14C]bentazon by BASF (Ludwigshafen, FRG). [phenyl-U-14C]Chlortoluron, [phenyl-U-14C]isoproturon, and [triazine-U-14C]simazine were generous gifts from Novartis (Basel, Swizerland). [phenyl-U-14C]-2,4-Dichlorophenoxyacetic acid was purchased from Sigma.Plant Material--
Jerusalem artichoke (H. tuberosus
L. var. Blanc commun) tubers were grown in open field, harvested in
November, and stored in plastic bags at 4 °C in the dark. For aging
experiments, tubers were sliced (1.5 mm thick), washed, and aged for
48 h in aerated (4 liters·min1) distilled water
containing 20 mM of aminopyrine, 8 mM sodium phenobarbital, or 25 mM MnCl2. The
MnCl2 solution was adjusted to pH 7.
RNA Isolation and RNA Blot Hybridization--
Total RNA were
isolated as described by Lesot et al. (28). Denatured RNA
was separated in the presence of formaldehyde through a 1.2% agarose
gel and transferred onto a nylon membrane Hybond N+,
Amersham Pharmacia Biotech. RNA blots prehybridization and
hybridization with a probe, radiolabeled with 50 µCi of
[-32P]dCTP by random priming, were carried out at
65 °C according to established procedures (29). Membranes were
washed twice for 10 min with 2× SSC, 0.1% SDS and once for 10 min
with 0.2× SSC, 0.1% SDS at room temperature, then twice for 30 min
with 0.2× SSC, 0.1% SDS at 55 °C. The hybridization signal was
recorded by autoradiography. RNA amounts were standardized by
hybridization at 55 °C to a 300-bp Capsicum annuum 25 S
rRNA probe.
cDNA Library and Screening--
Poly(A)+ RNAs
were prepared from H. tuberosus tuber tissues sliced and
aged 24 h in the presence of 20 mM aminopyrine (28). A
cDNA library was constructed in the vector -ZAPII (Stratagene), starting from 5 µg of polyadenylated RNA, according to the
manufacturer's instructions. Approximately 2 × 105
plaque-forming units were screened with antibodies raised against a
P450-enriched fraction purified from MnCl2-induced tuber
tissues (27), using alcaline phosphatase detection. Fifty-six positive clones were isolated. They were tested for the presence of a P450 consensus sequence using the
PCR1 approach previously
described by Meijer et al. (30). PCR-amplified DNA fragments
were obtained from 15 clones. They were reamplified, radiolabeled, and
hybridized with total RNA from dormant, wounded, and
aminopyrine-treated tissues. Four of them (1D, 12B, 13B, and 13C)
hybridized to transcripts of the expected size (1.6-2.3 kb). The
corresponding clones were purified by low density screening, before
rescuing pBluescript phagemids. Sequencing of the inserts showed that
only 1D coded for a P450 missing about 510-540 nucleotides at the
5'-end. Rescreening of the library (6.105 plaque-forming
units) with the radiolabeled 1D probe was performed at high stringency
(65 °C) according to established procedures (29). Membranes were
washed twice for 10 min with 2× SSC, 0.1% SDS and once for 10 min
with 0.2× SSC, 0.1% SDS at room temperature, then once for 30 min
with 0.2× SSC, 0.1% SDS at 55 °C. Hybridization signal was
recorded by autoradiography. The inserts of 216 positive plaques were
PCR-analyzed for size and hybridization. Ten clones were selected and
rescreened under the same conditions before rescuing pBluescript
phagemids and sequencing the inserts. Comparison of the longest insert
(1DN) with P450 sequences available in data banks indicated that it was
still missing 10-20 coding nucleotides. The missing nucleotides were
obtained using the 5'-RACE system from Life Technologies, Inc.,
according to manufacturer's instructions, and using
poly(A)+ RNA isolated from H. tuberosus tubers
treated with 20 mM aminopyrine. Amplified cDNA was
cloned in a pGEM-T vector (Promega) according to the manufacturer's
instructions, and eight bacterial colonies were analyzed for the
presence of the missing fragment. Two putative 5'-end sequences were
thus identified. Both DNA fragments were ligated to the partial 1DN
using a unique Tth111 site present in the overlapping sequence to
reconstitute full-length cDNAs.
Yeast Expression--
BamHI and EcoRI
sites were introduced by PCR just upstream of the ATG and downstream of
the stop codon of the full-length coding sequences,
respectively, using the primers 5'-ATATATGGATCCATGGAGATCCCATATCTACTCACC (sense) and 5'-TATATAGAATTCGACTCACAGTTCGGACAGTAGATTCGTCATC (reverse). The PCR mixture was preheated for 2 min at 92 °C before addition of
1 unit of Pfu DNA polymerase (Stratagene). After 3 min of
additional heating at 92 °C, 30 cycles of amplification were carried
out as follows: 1-min denaturation at 92 °C, 1-min annealing at
52 °C, and 2-min extension at 72 °C. The reaction was completed
by 10-min extension at 72 °C. After
BamHI/EcoRI digestion, the 1515- and 1560-bp
coding sequences were inserted into the vector pYeDP60 (31).
Saccharomyces cerevisiae strains W(R), WAT21, and WAT11 and
transformation and yeast growth media were described by Pompon et
al. (31). A colony from a SGI plate was transferred into 50 ml of
SGI medium and grown at 30 °C for 46 h. Cells were recovered by
10-min centrifugation at 8000 × g, washed with 25 ml
of YPI medium, and resuspended in 225 ml of YPI. Galactose induction was carried out for 14-16 h with shaking at 160 rpm, until cell density reached 2.5 × 107 cells·ml1.
When indicated, 0.5 mM
-aminolevulinic acid
methyl ester (Sigma) was added to the induction medium. Cells were
either used directly or stored at 4 °C for 24 h before
preparation of the microsomes as described by Pierrel et al.
(32) with addition of 1% serum albumin, 2 mM
-mercaptoethanol, 10 mM sodium disulfite, and 1 mM phenylmethylsulfonyl fluoride to the extraction
buffer.
Analytical Methods and Enzyme Assays-- Fatty acid metabolism was assayed as in Pinot et al. (33). Metabolites were resolved by thin layer chromatography (Silica Gel G60 F252, 0.25 mm, Merck) with a mixture of diethylether/light petroleum (boiling point, 40-60 °C)/formic acid (70:30:1, v/v/v) for C10 to C14 fatty acids, or a mixture of the same solvents (50:50:1) for long chain fatty acids. The areas corresponding to polar metabolites generated from each substrate were scrapped directly into counting vials or eluted with diethylether and subjected to reverse phase-HPLC analysis using a mixture of water/acetonitrile/acetic acid (25:75:0.2) and (45:55:0.2) as described previously (23, 33). Radioactivity of reverse phase-HPLC effluents was monitored with a computerized on-line solid scintillation counter (Ramona-D RAYTEST, Germany). The fluorimetric assays for 7-alkoxycoumarins and 7- alkoxyresorufins O-dealkylation were described in Werck-Reichhart et al. (34). Tests of diclofop, 2,4-dichlorophenoxyacetic acid, chlorsulfuron, and chlorotoluron metabolism were carried out as described by Zimmerlin et al. (19). Tests of isoproturon and simazine metabolism were as for chlortoluron, except TLC solvents were hexane/chloroform/acetone/ethanol 8:8:4:1 (v/v/v/v) and dichlorometane/methanol/formic acid 90:10:3 (v/v/v), respectively. Assay of bentazon ring-hydroxylation was described in McFadden et al. (35), trans-cinnamate 4-hydroxylation in Reichhart et al. (36), and benzoate 2-hydroxylation in Pierrel et al. (32). Geraniol and abscisic acid hydroxylation were tested according to Vetter et al. (37) and Gillard and Walton (38), respectively.
Spectrophotometric measurements of P450 content were performed as in Gabriac et al. (39). Protein was quantified using the Bio-Rad protein assay. The data are means ± S.D. of triplicate determinations.Sequence Analysis and Comparison-- Double-stranded pBluescript subclones were sequenced using the prism Ready Reaction dye deoxy terminator cycle method of Applied Biosystems Inc. The sequence data were analyzed using the GCG sequence analysis software package, version 8.1 (40). Sequences were aligned using ClustalW (41) to avoid insertion of gaps in hydrophobic helices. The alignment refined by hand and displayed using SeqVu 1.0.1. (Garvan Institute, Sydney). The tree was drawn using Treeview (42).
Gas Chromatography-Mass Spectrometry Analysis--
The
oxygenated metabolites of fatty acids were purified by TLC, methylated
with diazomethane, and silylated with a mixture of
bis-(trimethylsilyl)trifluoroacetamide + 1% trimethylchlorosilane and
pyridine (1:1; v/v), before gas chromatography and electron impact (70 eV) ionization mass spectrometry. The analysis was monitored on a 1%
SE30 capillary column (30 m × 0.025 mm) programmed to rise from
100 to 280 °C at 6 °C·min1, coupled to a LKB 900S
mass spectrometer with an LKB 2130 computer on line.
![]() |
RESULTS |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
Isolation of the CYP81B1 cDNA-- We previously raised antibodies against a P450-enriched fraction partially purified from MnCl2-induced H. tuberosus tuber tissues (27). These antibodies inhibited lauric acid in-chain hydroxylation by about 30%. They were used to screen a cDNA library prepared from tuber tissues treated for 24 h with aminopyrine to induce fatty acid hydroxylase activity. Fifty-six positive clones were isolated and tested for the presence of a P450 consensus sequence using the PCR technique previously described by Meijer et al. (30). PCR fragments of expected size were obtained from 15 clones, labeled, and hybridized with total RNA prepared from dormant, wounded, or aminopyrine-treated tuber tissues. One of the 15 clones corresponded to a transcript of approximately 1.7 kb, which was undetectable in dormant tuber, became detectable in wounded tissues, and clearly accumulated following treatment with aminopyrine, MnCl2, or phenobarbital (Fig. 1). Sequencing of its insert showed that it coded for a typical P450 missing about 500 nucleotides encoding the N terminus. Rescreening of the library with this insert as a probe led to obtaining the 1DN cDNA still lacking a start codon (Fig. 2), but missing less than 50 nucleotides according to alignment with sequences available in data bases. When submitted to the P450 nomenclature committee (c/o Dr. D. R. Nelson, University of Tennessee, Memphis), the polypeptide encoded by 1DN was assigned to a new P450 subfamily and named CYP81B1.
|
|
Obtention of Full-length Sequences-- Unexpectedly, the 5'-RACE experiment performed to obtain the missing nucleotides led to the isolation of two cDNA fragments: "s" (376 bp) and "l" (421 bp), both with an ATG start codon preceded by the same 5'-noncoding sequence. s differed from l by two insertions of 14 and 1 amino acids only present in l, two nonconservative amino acid changes, and two silent nucleotide modifications (Fig. 2). It seems unlikely that such a difference could result from a PCR artifact. The N terminus forms the major membrane anchoring segment of P450 proteins. Different membrane anchors may thus reflect different subcellular localizations of two closely related proteins. Comparison of s and 1DN showed that they were identical in their overlaping sequence, and that 1DN was missing only 5 bp from the full-length coding sequence. Two full-length coding sequences were reconstituted from 1DN and s or l, to obtain CYP81B1s (1518 bp; EMBL accession no. AJ000477) and CYP81B1l (1563 bp; EMBL accession no. AJ000478) coding for 505 and 520 amino acids, respectively.
Characteristics of the CYP81B1 Proteins-- The CYP81B1s cDNA encodes a protein of predicted Mr 57,060 with a pI of 7.86. In the case of the CYP81B1l construction, the Mr is shifted to 58,877 and the pI to 8.06. In addition to typical Mr and pI, CYP81B1 displays all the signatures of P450 proteins. The PFG(ASV)GRRXC(PAV)G sequence, characteristic of plant P450s from the group A (as defined by Durst and Nelson (43)) and involved in heme binding, is found as expected near the C terminus (Fig. 2). The consensus (AG)GX(DE)T(TS), typical of the I helix that participates in oxygen binding and charge transfer in the active site, is also present at the expected location. The N-terminal segment of CYP81B1 is somewhat unusual due to a high content in hydroxylated residues (S and T) and to repetitive alternation of such residues with stretches of hydrophobic amino acids, in particular in CYP81B1l. It can be speculated that the unusual structure of this membrane anchoring segment is related to some particular location of the protein in a specialized cellular compartment or membrane domain. The cluster of basic residues acting as halt-transfer signal and the proline-rich hinge region expected in endoplasmic reticulum bound P450s are present in CYP81B1.
That CYP81B1 belongs to the A group of typical plant P450s is confirmed by the comparison of its overall amino acid sequence with proteins of other organisms. CYP81B1 belongs to the same family as CYP81A2 (44% amino acid identity) and show high local identities to the C-terminal region of the partial CYP81A1, A3, and A4 (46-56% overall identity) isolated from maize (44) (Fig. 3). The other most closely related proteins all belong to the group A of plant P450s, CYP82A1 from pea (40% identity), CYP92A2 from Nicotiana tabacum (38% identity), CYP71A1 from avocado (37% identity), and CYP93A1 from soybean (36% identity). The function of all these related enzymes is still unknown. CYP81B1 has only a 34% amino acid identity with the xenobiotic metabolizing CYP76B1 and 29% identity with the cinnamate 4-hydroxylase (CYP73A1) previously isolated from H. tuberosus (45, 46). It shows no phylogenic relatedness to any of the fatty acid-metabolizing enzymes described so far (Fig. 4).
|
|
Optimized Expression in Yeast--
Fig.
5 compares the level of expression of
CYP81B1s and CYP81B1l in three engineered yeast strains, W(R), WAT11,
and WAT21, which overexpress either the endogenous yeast P450 reductase
or the Arabidopsis thaliana P450 reductases ATR1 and ATR2,
respectively (47). Expression of CYP81B1 and of the different
reductases was under the transcriptional control of the artificial
galactose-inducible promoter GAL10-CYC1. After 16 h of
induction with galactose, no P450 was detected in microsomes prepared
from the W(R) strain transformed with either CYP81B1s or
CYP81B1l. In contrast, P450 accumulation was observed in
microsomes from WAT11 and WAT21 transformed with either of the two
constructions (Fig. 5). P450 contents were higher in WAT11 than in
WAT21: 145 ± 11 versus 118 ± 9 pmol·mg1 for CYP81B1s and 40 ± 7 versus 19 ± 5 pmol·mg
1 protein for
CYP81B1l. Both the length of the membrane anchoring sequence, and the
nature of the reductase present in microsomes thus seem to determine
the level of CYP81B1 expression in yeast. The most plausible
interpretation of these results is that CYP81B1 in yeast microsomes is
very labile and that a short membrane-spanning sequence and
co-expressed ATR1 both improve the enzyme stability. CYP81B1s recovery
from WAT11 was further increased, up to 215 pmol·mg
1
protein, by keeping the culture standing at 4 °C for 24 h
before preparing the microsomes. The yield in CYP81B1l was, however, not increased by this treatment. Addition of
-aminolevulinic acid to
the induction medium had no effect on the level of expression of
CYP81B1.
|
CYP81B1 Is a Fatty Acid Hydroxylase--
Microsomes prepared from
WAT11 expressing CYP81B1s or CYP81B1l were used to assay catalytic
activity. The molecules tested as substrates are listed in Table
I. They include phenolics that are known
or potential substrates of P450 enzymes in H. tuberosus, isoprenoids, herbicides, and eight of the most common fatty acids found
in higher plants. A rapid conversion into polar metabolites was
obtained with only capric, lauric, and myristic acids. The formation of
these polar metabolites was dependent on CYP81B1 as shown in Fig.
6 for lauric acid; metabolism required
the presence of NADPH and was not detected with membranes of yeast
transformed with a void plasmid. All three fatty acids were metabolized
with similar and very high efficiencies (Table
II). In addition to fatty acid
metabolism, a very low chlortoluron ring-methyl hydroxylase activity was detected (kcat ~0.09
min1 for CYP81B1s) in microsomes from transgenic
yeast.
|
|
|
Compared Function and Coupling of CYP81B1s and CYP81B1l-- Previous reports have indicated that changes in the anchoring N-terminal segment of membrane-bound P450s has no critical effect on the catalytic activity and substrate specificity (48-50). This was confirmed by our experiments. The same compounds were metabolized by microsomes prepared from yeast expressing CYP81B1s or CYP81B1l (Table I), although higher specific activities were always measured with CYP81B1s.
The data available so far suggest the existence of multiple P450 reductases in many plant species (43). The specific functions of these multiple reductases has not yet been determined. They may be targeted to different subcellular compartments or membrane subdomains or their differences may just be functional and favor electron transfer to specific P450 proteins. Table III compares the capric acid hydroxylase activity of the s and l constructs in microsomes from yeast strains overexpressing different P450 reductases. No activity was measured in the microsomes from the W(R) strain, which overexpresses yeast reductase, in agreement with the absence of detectable CYP81B1 expression in this strain. The CYP81B1s construct was about 50% more active in the presence of the A. thaliana reductase ATR1 than in the presence of ATR2. By contrast, the specific activity of CYP81B1l was 67% higher in the presence of ATR2 than with ATR1. Different expression of ATR1 and ATR2 reductases does not seem to account for the differences in hydroxylase activity, since NADPH-dependent cytochrome c reduction measured in microsomes from WAT11 and WAT21 was quite similar when the strains were transformed with CYP81B1s (2.92 ± 0.03 and 3.18 ± 0.09 nmol s
|
Regiospecificity of the Fatty Acid Hydroxylation--
Fig. 6 shows
that the same metabolites were produced by microsomes prepared from
CYP81B1-transformed yeast and from aminopyrine-treated H. tuberosus tuber. Previous data indicated that several
oxygenated derivatives of lauric acid were formed by plant microsomes.
They were characterized as the 8-, 9-, and 10-hydroxylated products (21). Gas chromatography-mass spectrometry analysis of the polar metabolites generated from the three fatty acid substrates by CYP81B1
led to the characterization of complex mixtures of monohydroxylated products. In the case of lauric acid, the major methylester
trimethylsilyl ether derivatives showed the expected mass fragmentation
for hydroxylated fatty acids, with characteristic ions resulting from
,
cleavage of trimethylsilyl ether at m/z 131 and 273 for the 10-hydroxy acid, m/z 145 and 259 for the 9-hydroxy
acid, and m/z 159 and 245 for the 8-hydroxy acid. Similarly,
fragmentation ions of the major metabolites were characteristic of 9-, 8-, and 7-hydroxylated (m/z 117 and 259, m/z 131 and 245, and m/z 145 and 231) products in the case of capric
acid, and of 11-, 10-, and 9-hydroxylated (m/z 145 and 287, m/z 159 and 273, and m/z 173 and 259) fatty acids
for myristic acid. The major metabolites were the 9-hydroxy derivatives
for capric and lauric acids, and the 10-hydroxylated myristic acid. The
best HPLC and gas chromatography resolution of metabolites was obtained
for lauric acid. In this case, the estimated ratio of the 10-, 9-, and
8-hydroxylated products was 21/64/15. This is very similar to the
ratios measured with plant microsomes and suggests that CYP81B1 is the
sole medium chain metabolizing P450 in H. tuberosus tuber
tissues.
![]() |
DISCUSSION |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
A characteristic of P450-dependent fatty acid hydroxylases in higher plants is a very low activity in normal plant tissues (tuber or young shoots). Small increases in activity are observed after mechanical stress, such as wounding or aging of the shoots or tissues, but these increases are negligible compared with the response to some specific chemical treatments (15). This property has been exploited for the isolation of the cDNA coding for H. tuberosus fatty acid in-chain hydroxylase. Hydroxylase activity is very low in dormant or wounded tuber tissue, but is strongly induced by MnCl2 or aminopyrine (22, 24). We thus combined use of antibodies directed against partially purified MnCl2-induced P450s, screening of a library from aminopyrine-treated tissues and selection of clones coding aminopyrine-induced transcripts to isolate the CYP81B1 cDNA. This is the first example of isolation of a plant P450 gene of defined function on the basis of chemically induced expression. Another successful approach taking advantage of differential gene expression has been previously reported (51). It was using a combination of PCR on conserved P450 sequences and selection on the basis of developmental expression, and led to isolation of sequences coding flavonoid hydroxylases involved in the biosynthesis of anthocyanins.
Functional characterization, but also detailed analysis of the substrate-specificity and regioselectivity of CYP81B1 was made possible by the expression of the enzyme in yeast. The yeast expressed protein catalyzes in-chain hydroxylation of C10:0, C12:0, and C14:0 fatty acids. The three substrates are metabolized with high and comparable efficiencies. Shorter fatty acids are also possible substrates; short chain acids being volatile molecules, their metabolism was not assayed. Long chain saturated or unsaturated fatty acids, however, have been assayed. They were not metabolized. Neither were the isoprenoids (geraniol, abscisic acid), aromatic molecules, and herbicides tested in our experiments. CYP81B1 thus seem highly specific for medium chain fatty acids. The high affinity of the enzyme for these molecules (in the 100 nM to 1 µM range) would suggest that they are its natural substrates. From the data obtained with plant microsomes it can be assumed that CYP81B1 is also able to epoxidize or hydroxylate medium chain unsaturated fatty acids (25, 26). Some of the unsaturated acids seem to be attacked with a high stereospecificity. Such molecules would be good potential natural substrates of CYP81B1. Nothing is known, however, concerning the possible physiological function of in-chain hydroxylated or epoxidized medium chain fatty acids.
Analysis of the metabolites of capric, lauric, and myristic acids
showed that a complex mixture of in-chain monohydroxylated derivatives
was generated by CYP81B1. This is probably indicative of some mobility
of the molecules in the active site, and could be taken as an argument
for the saturated medium chain fatty acids not being the physiological
substrates. The major site of attack is at carbon 9 (capric and lauric
acid) or 10 (myristic acid) depending on the length of the aliphatic
chain. The regioselectivity of the attack thus seems to be primarily
determined by the distance relative to the carboxyl end of the
molecule. The small influence of the distance to -terminus would be
easily explained if the
-terminal methyl was maintained curled away
and stuck in a hydrophobic patch of the protein located above heme as
in the fatty acid-bound BM-3 structure (52), since the distance of
attack to the COOH terminus would increase with the overall bend of the
molecule.
Our results demonstrate that a single P450 catalyzes the in-chain
hydroxylation of C10:0, C12:0, and C14:0 fatty acids, and that several
monohydroxylated positional isomers are generated from the three fatty
acids by the same protein. This new P450 is typical from higher plants,
and has no known equivalent in other living organisms. One complete and
three partial sequences coding for ethanol-induced P450s belonging to
the same family (but to another subfamily) have been isolated from
etiolated maize shoots (44). The function of these genes has never been
determined. It is, however, noteworthy that lauric acid in-chain
hydroxylase activity has been detected in maize shoots (17). Two
self-sufficient bacterial and fungal cytochromes P450, CYP102 or
P450BM-3 from Bacillus megaterium and P450foxy
from Fusarium oxysporum, are able to perform in-chain
hydroxylation of medium chain fatty acids (53, 54). They differ from
CYP81B1 in regiospecificity and substrate specificity. Both enzymes
produce -1 to
-3 hydroxylated metabolites. They hydroxylate long
chain as well as medium chain fatty acids. In addition, their
Km values for fatty acids are in the 10 to 200 µM range.
In terms of amino acid sequence, CYP81B1 completely differs from the
plant, bacterial, fungal, and animal fatty acid oxygenases already
characterized. It shares less than 30% identity to other plant P450
enzymes, such as allene oxide synthases and fatty acid hydroperoxide
lyases (CYP74s) and the small CYP94 family of fatty acid
-hydroxylases recently isolated in our laboratory.2 It
also greatly differs from the bacterial CYP102 and from the proteins of
the CYP4 family (
and
-1 hydroxylases) present in insects and
mammals, and from the different hydroxylases and epoxydases of the
mammalian CYP2 family involved either in medium-chain fatty acid
-1
hydroxylaltion or the arachidonic cascade and in the synthesis of
signaling molecules (55, 56). The oleate 12-hydroxylase, which
synthetizes ricinoleic acid in castorseed, is a totally different
enzyme both from a mechanistic and phylogenetic point of view and is
related to fatty acyl desaturases (57).
CYP81B1 is thus a new and very interesting tool for the modification of fatty acid content of oilseeds and for the orientation of lipid synthesis toward the production of oxygenated derivatives. Redirection of fatty acid synthesis to medium chains in seeds of Arabidopsis or rapeseed has been successfully achieved. Plants were transformed with genes coding acyl-carrier protein thioesterases specific for medium chain acyl-acyl carrier protein isolated from plants accumulating unusual fatty acids such as California bay or Cuphea spp. (3, 58, 59). Combined transformation with CYP81B1 under the control of a seed specific promoter could lead to the production of in-chain hydroxy fatty acids of specific lengths. CYP81B1 has the advantage not to attack the most common C16 and C18 constituents of plant membrane lipids. Its partial lack of substrate specificity could be largely compensated by the higher specificity of the thioesterases.
In summary, we have taken advantage of Mn2+ and
aminopyrine inducibility to isolate a cDNA (CYP81B1)
coding the in-chain hydroxylase of C:10, C:12, and C:14 fatty acids in
higher plants. We demonstrate that the same yeast expressed enzyme
catalyzes primarily the formation of the -1,
-3, and
-4
monohydroxylated products of capric, lauric, and myristic acids,
respectively. This P450 is highly specific for fatty acids and does not
metabolize herbicides or aromatic molecules. This new P450 is a
potential tool to redirect lipid synthesis in oilseed crops toward
production of oxygenated medium chain fatty acids.
![]() |
ACKNOWLEDGEMENTS |
---|
We thank Drs. D. Pompon and P. Urban for providing the W(R), WAT11, and WAT21 yeast strains and the pYeDP60 expression vector and Dr. R. DeRose (Rhône-Poulenc Agro, Lyon) for help in the construction of the cDNA library. We also thank M. F. Castaldi for technical assistance. The critical reading of the manuscript by F. Bernier is gratefully acknowledged.
![]() |
FOOTNOTES |
---|
* This work was supported in part by the Convention GREG/INRA "Complémentation de la levure par des gènes de plantes."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.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) AJ000477 (CYP81B1s) and AJ000478 (CYP81B1l).
These two authors contributed equally to this work.
§ Supported by a postdoctoral grant from the Spanish Ministerio de Agricultura, Pesca y Alimentacion.
¶ Supported by the Ministére de la Recherche et de l'Enseignement Supérieur.
To whom correspondence should be addressed. Tel.:
33-3-8835-8332; Fax: 33-3-8835-8484; E-mail: daniele.werck{at}ibmp-ulp.u-strasbg.fr.
1 The abbreviations used are: PCR, polymerase chain reaction; RACE, rapid amplification of cDNA ends; HPLC, high performance liquid chromatography; bp, base pair(s); kb, kilobase pair(s).
2 I. Benveniste, personal communication.
![]() |
REFERENCES |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|