Suppression of Leukotriene Formation in RBL-2H3 Cells That
Overexpressed Phospholipid Hydroperoxide Glutathione
Peroxidase*
Hirotaka
Imai
,
Kazuki
Narashima
,
Masayoshi
Arai
,
Hikaru
Sakamoto
,
Nobuyoshi
Chiba§, and
Yasuhito
Nakagawa
¶
From the
School of Pharmaceutical Sciences, Kitasato
University, 5-9-1 Shirokane, Minato-ku, Tokyo 108 and
§ Japan Energy Corporation,
3-17-35 Niizo-Minami, Toda-shi, Saitama 335, Japan
 |
ABSTRACT |
The overexpression of phospholipid hydroperoxide
glutathione peroxidase (PHGPx) by RBL-2H3 cells was used as the basis
for an investigation of the effects of PHGPx on the formation of
leukotrienes. The rates of production of leukotriene
C4 (LTC4) and leukotriene B4
(LTB4) in cells that overexpressed PHGPx were 8 times lower than those in a control line of cells. The reduction in rates of
production of leukotrienes apparently resulted from the
increase in the PHGPx activity since control rates of formation of
leukotrienes could be achieved in PHGPx-overexpressing cells upon
inhibition of PHGPx activity by diethyl malate. The conversion of
radioactively labeled arachidonic acid to intermediates in the
lipoxygenase pathway, such as 5- hydroxyeicosatetraenoic acid
(5-HETE), LTC4, and LTB4, was strongly
inhibited in PHGPx-overexpressing cells that had been prelabeled with
[14C]arachidonic acid. PHGPx apparently inactivated the
5-lipoxygenase that catalyzed the conversion of arachidonic acid to
5-hydroperoxyeicosatetraenoic acid (5-HPETE) since 5-HPETE is a common
precursor of 5-HETE, LTC4, and LTB4. The rates
of formation of LTC4 and LTB4 in
PHGPx-overexpressing cells returned to control rates upon the addition
of a small amount of 12-HPETE. Flow cytometric analysis revealed that
the rapid burst of formation of lipid hydroperoxides induced by A23187
was suppressed in PHGPx-overexpressing cells as compared with the control lines of cells. Subcellular fractionation analysis showed that
the amount of PHGPx associated with nuclear fractions from PHGPx-overexpressing cells was 3.5 times higher than that from the
control line of cells. These results indicate that PHGPx might be
involved in inactivation of 5-lipoxygenase via reductions in levels of
the fatty acid hydroperoxides that are required for the full activation
of 5-lipoxygenase. Thus, in addition to its role as an antioxidant
enzyme, PHGPx appears to have a novel function as a modulator of the
production of leukotrienes.
 |
INTRODUCTION |
Leukotrienes are important mediators both in host defense
mechanisms and in inflammatory disease states since they have potent effects on cell migration, muscle contraction, vascular permeability, and the release of lysosomal enzymes (1-3). Leukotrienes can be formed
in mast cells, granulocytes, and monocytes/macrophages in response to
extracellular stimulation. The biosynthesis of leukotrienes is
initiated by the release of arachidonic acid from membrane
phospholipids (4). The liberated arachidonic acid is oxidized to
hydroperoxyeicosatetraenoic acid
(5-HPETE)1 and subsequent
dehydration yields an unstable epoxide intermediate, leukotriene
A4 (LTA4). These sequential reactions are
catalyzed by 5-lipoxygenase that is the primary enzymatic regulator of
the biosynthesis of leukotrienes (5). LTA4 is further
converted to a variety of leukotrienes, such as LTB4 and
LTC4. The nuclear membrane is the site of leukotriene
synthesis, and cytosolic phospholipase A2 and
5-lipoxygenase are translocated to this site from the cytosol after the
activation of cells (6, 7). The activity of 5-lipoxygenase is regulated
by several factors, such as Ca2+, ATP, and
5-lipoxygenase-activating protein (FLAP) (8-12). There is evidence
that fatty acid hydroperoxides might also activate 5-lipoxygenase
(13, 14). A requirement for fatty acid hydroperoxides in the activation
of lipoxygenase suggests that the activity of 5-lipoxygenase might be
regulated by its own product, namely 5-HPETE (15). Intracellular
5-HPETE can be reduced to 5-hydroxyeicosatetraenoic acid (5-HETE) by
lipid peroxidases such as glutathione peroxidase (GPx). However, the
lipid peroxidase responsible for the reduction of 5-HPETE remains to be
defined. This reduction seems to be a key reaction in the control of
the production of leukotrienes since it can determine the level of
5-HPETE, which is utilized as an activator of 5-lipoxygenase and as a
precursor of LTA4.
GPx reduces cellular lipid hydroperoxides. Two types of
selenium-dependent GPx are widely distributed in various
tissues. Cytosolic glutathione peroxidase (cGPx, GPx1) is predominantly present in the cytosol of tissues, and it reduces fatty acid
hydroperoxides and H2O2 at the expense of
glutathione (16). Phospholipid hydroperoxide glutathione peroxidase
(PHGPx, GPx4) is localized in both the cytosol and the membrane
fraction (17). PHGPx can directly reduce the phospholipid
hydroperoxides, fatty acid hydroperoxides (18, 19), and cholesterol
hydroperoxides (20) that are produced in peroxidized membranes and
oxidized lipoproteins. Although direct evidence for the involvement of
GPx in the reduction of 5-HPETE, required for the activation of
5-lipoxygenase, is still lacking, it has been shown that impairment of
GPx activity by selenium deficiency or glutathione depletion leads to
enhanced activity of 5-lipoxygenase in rat polymorphonuclear
leukocytes, rat basophile leukemia cells (RBL-1) (21), B lymphocytes
(22, 23) and human granulocytes (24, 25). These results suggest that
glutathione peroxidase might regulate the activity of 5-lipoxygenase in
the cellular level. The question now arises as to whether cGPx or PHGPx
might be responsible for the regulation of the formation of
leukotrienes. We are interested in the possible role of PHGPx in the
regulation of leukotriene synthesis since PHGPx is unique as an isozyme
of GPx, being able to interact with the nuclear membrane in which the
synthesis of leukotrienes occurs.
Stable transfectants that overexpress PHGPx provide useful model
systems with which to attempt to clarify the ability of PHGPx to
modulate leukotriene synthesis. We reported previously the cloning of a
cDNA for rat PHGPx (26, 27) and the establishment of
PHGPx-overexpressing stable transfectants of rat basophile leukemia 2H3
(RBL-2H3) cells (28). PHGPx-overexpressing cells exhibit resistance to
cell death that is due to oxidative damage. RBL-2H3 cells are a
neoplastic cell line from rats. They are derived from basophiles, which
are among the cells that have been used most extensively in studies of
5-lipoxygenase. RBL-2H3 cells produce LTC4 and
LTB4 predominantly in response to stimulation by calcium ionophores (29, 30).
In the present study, the PHGPx-overexpressing RBL-2H3 cells were used
to examine the effects of PHGPx on the formation of leukotrienes. We
showed that PHGPx significantly suppressed the production of
leukotrienes via a reduction in the level of intracellular lipid
hydroperoxides, which was due to suppression of the activity of
5-lipoxygenase.
 |
EXPERIMENTAL PROCEDURES |
Reagents--
Antibodies against PHGPx were prepared previously
(28). Antibodies against 5-lipoxygenase and FLAP were a kind gift from Dr. M. Murakami (Showa University, Tokyo) (31). Anti-histone H1
monoclonal antibodies and 125I-protein A (2.60-3.70 TBq/g)
were purchased from Cosmobio Co. Ltd. (Tokyo, Japan) and ICN
Biochemicals Inc. (Irvine, CA), respectively. Antibodies against
cPLA2, diethyl malate (DEM), LTB4,
LTC4, LTA4 methyl ester, A23187, and
5,6-carboxy-2
,7
-dichlorofluorescein-diacetate (DCFH-DA) were obtained
from Funakoshi Co. Ltd. (Tokyo, Japan).
Cell Cultures--
RBL-2H3 cells that overexpressed PHGPx were
generated by transfection with pSR
-PHGPx and pSV2neo as described
previously (28). In brief, fragments of a rat cDNA for PHGPx,
namely the insert in pRPHGPx2 (761 base pairs) (26), were subcloned
into pSR
as the expression vector (32). RBL-2H3 cells were harvested by trypsinization and were resuspended in the Dulbecco's modified essential medium that contained 20 mM HEPES, 2 mM glutamine, penicillin (100 units/ml), and streptomycin
(100 units/ml) at a concentration of 4 × 107
cells/ml. The suspension of cells (0.25 ml) was transferred to an
electroporation cuvette (0.4-cm gap; Bio-Rad) with a total of 20 µg
of linearized DNA, which consisted of 18 µg of SR
-PHGPx and 2 µg
of pSV2neo (33). The latter plasmid was used to confer resistance to
G418 (Geneticin; Life Technologies, Inc.). A charge of 250 V at 500 microfarads was applied at room temperature with a Gene Pulser II
(Bio-Rad), and after a 10-min recovery period, the culture of the cells
was reinitiated. Selection with G418 (1 mg/ml) was initiated after
24 h, and cells were subsequently exposed to 1 mg/ml G418 for 2 weeks. Individual G418-resistant colonies were isolated with cloning
cylinders. G418-resistant cells were analyzed by immunoprecipitation
with antibodies against PHGPx (anti-PHGPx) to determine the level of
expression of PHGPx 10 days after transfection. Control lines of cells
were prepared by transfection with pSV2neo and pSR
that did not
contain an insert of PHGPx cDNA.
Labeling with 75Se of RBL-2H3
Cells--
[75Se]Sodium selenite (10 mCi/mg; Amersham
Corp., Little Chalfont, Buckinghamshire, UK) was used to label the
selenoproteins of RBL-2H3 cells. PHGPx-overexpressing RBL-2H3 cells
(5 × 106 cells) were labeled with 140 nCi/ml
[75Se]sodium selenite for 96 h. Labeled cells
were collected after washing with ice-cold phosphate-buffered saline
and sonicated in 1 ml of 10 mM Tris-HCl buffer (pH 7.4)
containing 5 mg/ml leupeptin and 17 mg/ml phenylmethylsulfonyl fluoride
(PMSF). The homogenate was centrifuged at 10,000 × g
for 10 min at 4 °C, and the supernatant was collected for the
analysis of selenoproteins. Labeled selenoproteins in transformants
were separated by SDS-PAGE (12.5% acrylamide gel) under non-reducing
conditions, as described by Laemmli (34). Gels were stained for 10 min
with 0.1% (w/v) Coomassie Brilliant Blue R that had been dissolved in
glacial acetic acid, methanol, and water (10:40:50, v/v). Bands of
dried gels were analyzed densitometrically with a Bio-Imaging Analyzer
(BAS2000; Fuji Film, Co. Ltd., Tokyo, Japan).
Immunoblot Analysis--
Cell homogenates and nuclear fractions
were fractionated by SDS-PAGE on 12.5% acrylamide gels and transferred
to PVDF membrane filter (Millipore Co., Bedford, MA) at 50 V for 150 min in 25 mM Tris, 192 mM glycine, 10% (w/v)
methanol at 4 °C in a protein transfer system (Bio-Rad), as
described previously (35). Each PVDF membrane with blotted protein was
blocked by incubation with 3% (w/v) skim milk in 10 mM
Tris-HCl (pH 7.4) that contained 150 mM NaCl and 0.1%
Tween 20 (TBS-T) for 1 h. The PVDF membrane was then incubated
with antiserum against cPLA2, 5-lipoxygenase, and FLAP that
had been diluted with TBS-T at an appropriate concentration for 2 h. Then the PVDF membrane was incubated for 1 h with horseradish peroxidase-conjugated goat antibodies against rabbit IgG or against mouse IgG (Zymed, South San Francisco, CA). The binding of antibodies to the antigen on the PVDF membrane was detected with an
enhanced chemiluminescence Western blotting analysis system
(Amersham Corp.).
Assays of Enzymatic Activities--
RBL-2H3 cells (2 × 107 cells) were sonicated in 1 ml of 10 mM
Tris-HCl buffer (pH 7.4) that included 5 mg/ml leupeptin and 17 mg/ml
PMSF. The homogenate was centrifuged at 10,000 × g for 10 min at 4 °C, and the supernatant was used for assays of enzymatic activity. PHGPx activity was measured as described previously (28). The
reaction mixture contained, in a final volume of 0.8 ml, 0.1 M Tris-HCl (pH 7.4), 5 mM EDTA, 1.5 mM sodium azide, 3 mM glutathione, 0.25 mM NADPH, 1 unit of glutathione reductase, 0.1% Triton
X-100, and 10 µM phosphatidylcholine hydroperoxide (PCOOH), which had been prepared from egg yolk phosphatidylcholine as
described previously (36). The reaction was started by the addition of
PCOOH at 37 °C after preincubation for 10 min. The rate of the
reaction was measured by following the decrease in the absorbance at
340 nm over a 10-min period. The reaction was stopped by the addition
of methanol, and the total lipids were extracted by the method of Bligh
and Dyer (37). The lipid extract was dried under a stream of nitrogen
gas, and the residue was dissolved in 0.05 ml of methanol. PCOOH
without reduction by PHGPx was quantitated by the methylene blue method
(38). The decrease in the amounts of PCOOH during the incubation was
calculated by subtracting the amounts of non-reduced PCOOH from the
original amount of PCOOH. cGPx activity was measured
spectrophotometrically by monitoring the decrease in absorbance at 340 nm with 0.25 mM hydrogen peroxide as substrate (39).
Glutathione S-transferase activity was measured
spectrophotometrically by monitoring the formation of the conjugate of
reduced glutathione and 1-chloro-2,4-dinitrobenzene at 340 nm (40).
Catalase activity was determined as described by Clairborne (41) with
10 mM hydrogen peroxide as the substrate.
Quantitation of LTB4 and LTC4 by Enzyme
Immunosorbent Assays (EIAs)--
RBL-2H3 cells (5 × 106 cells) were preincubated in phosphate-buffered saline
(PBS) that contained 1 mM CaCl2 for 10 min at 37 °C and then stimulated with 5 µM A23187 for 5 min.
Supernatants were prepared for the quantitation of LTB4 and
LTC4 by enzyme immunosorbent assays (EIAs; Amersham
Corp.).
Liberation of [14C]Arachidonic Acid from
A23187-stimulated Cells--
RBL-2H3 cells (4 × 104
cells) were grown in 24-well plates for 3 days. Cells then were
incubated with 0.1 µCi of [14C]arachidonic acid
(60-100 Ci/mmol; NEN Life Science Products) for 24 h at 37 °C.
Labeled cells were washed three times with PBS and then preincubated
with PBS that contained 1 mM CaCl2 for 10 min.
The cells that had been labeled with [14C]arachidonic
acid were stimulated with 5 µM A23187 for 15 min. After
centrifugation of samples to remove small amounts of dislodged cells
(20 s at 16,000 × g), supernatants were transferred to
scintillation vials, and radioactivity was determined by scintillation
counting (LS5000TD counter; Beckman Instruments, Fullerton, CA).
Release of radiolabeled arachidonic acid was expressed as the ratio of the radioactivity of arachidonic acid released into the culture medium
to the total radioactivity of cells multiplied by 100 to give a
percentage.
The Formation of LTC4 and LTB4 from
Exogenously Added LTA4--
LTA4 was prepared
by the hydrolysis of the methyl ester of LTA4 with 0.02 M lithium hydroxide at room temperature in darkness described previously (42, 43). Cells were incubated in the presence of
1 µM LTA4 for 10 min. The amounts of
LTC4 and LTB4 in the supernatant were
quantitated by EIAs.
The Formation of LTC4, LTB4, and 5-HETE
from Exogenous [14C]Arachidonic Acid--
RBL-2H3
cells (5 × 106 cells) were incubated with 0.1 µCi
of [14C]arachidonic acid for 24 h at 37 °C.
Labeled cells were stimulated with A23187 for 10 min in the presence of
1 mM CaCl2 as described above. After the
incubation, supernatants were obtained by centrifugation, and 3 ml of
ethyl acetate (pH 3.0), supplemented with 0.1 ml of 0.09 M
HCl, were added to each supernatant for the extraction of metabolites.
Non-labeled LTC4 (100 ng), LTB4 (100 ng), and 5-HETE (200 ng), as carriers, and prostaglandin B2
(PGB2; 50 ng) as an internal standard, were added before
the extraction. The supernatant was collected and injected into an HPLC
system equipped with a reverse-phase column (LiChrosorb RP-18; 240 × 0.4 mm inner diameter; Merck, Darmstadt, Germany) for the separation
of LTC4, LTB4, and 5-HETE. The mobile phase was
a mixture of acetonitrile, methanol, water, and acetic acid
(350:150:250:1, v/v). The flow rate was 1.0 ml/min with monitoring of
280 nm for LTC4, LTB4, and PGB2 and
at 235 nm for 5-HETE. Each 0.5 ml of fraction was collected for
measurement of radioactivity by scintillation counting.
Flow Cytometric Analysis of Intracellular Peroxides--
To
assess levels of intracellular peroxides, we performed flow cytometric
analysis using an oxidation-sensitive fluorescent probe,
5,6-carboxy-2
,7
-dichlorofluorescein-diacetate (DCFH-DA). After
preincubation with 12-HPETE and/or A23187, cells were washed with PBS
and incubated with 2.5 µM DCFH-DA in PBS for 30 min. DCFH-DA was deacylated to the non-fluorescent compound
2
,7
-dichlorofluorescein (DCFH) within the cells, and DCFH was
oxidized to the fluorescent compound 2
,7
-dichlorofluorescein by a
variety of peroxides (44). The fluorescent intensity of
dichlorofluorescein in the cells was analyzed with a flow cytometer
(EPICSR Elite Flow cytometer; Coulter, Hialeah, FL).
Subcellular Fractionation of
Cells--
[75Se]Sodium selenite-labeled cells were
fractionated by the previously described method with slight
modification (45). Cells were labeled with 140 nCi/ml
[75Se]sodium selenite for 96 h, and confluent cells
in 225-cm2 culture flask were washed 3 times with
phosphate-buffered saline and harvested with the aid of a rubber
policeman in phosphate-buffered saline. The cell suspension was
centrifuged at 800 × g for 10 min at room temperature.
The cell pellet was suspended in sucrose buffer (0.25 M
sucrose, 1 mM EDTA, 3 mM imidazole, and 0.1%
(v/v) ethanol (pH 7.2)) and centrifuged at 1,000 × g
for 10 min at 4 °C. Pellets of cells were resuspended in the sucrose
buffer at approximately 1 × 108 cells/ml. Leupeptin,
antipain, chymostatin, and pepstatin A were added at a final
concentration of 10 µg/ml each; PMSF was also added at a final
concentration of 100 µg/ml. Cells were homogenized with a
Teflon/glass Potter-Elvehjem homogenizer. The nuclear fraction (the
pellet) and a postnuclear fraction (the supernatant) were prepared by
centrifugation at 2,700 × g for 10 min. The nuclear fraction was suspended in 200 µl of the sucrose buffer.
Mitochondrial, microsomal, and cytosolic fractions from a postnuclear
fraction were obtained by differential centrifugation according to the method of de Duve et al. (45). The distribution of each
subcellular fraction was judged by standard enzymatic measurements,
cytochrome c oxidase (mitochondrial marker),
NADPH-cytochrome c reductase (microsomal marker), and
lactate dehydrogenase (cytosolic marker) as reported previously (27,
46). The distribution of histone H1 as nuclear marker in subcellular
fractions was determined by the immunoblotting with anti-histone H1
polyclonal antibody (47). Antibody bound was detected by
125I-protein A. The nuclear, mitochondrial, and microsomal
fractions were solubilized with 0.4% Triton X-100 in
phosphate-buffered saline for 2 h at 4 °C and centrifuged at
100,000 × g for 1 h at 4 °C. The supernatant
diluted with the same volume of PBS was immunoprecipitated with
anti-PHGPx as described previously (28). Immunoprecipitated proteins
were separated by SDS-PAGE (12.5% polyacrylamide) under non-reducing
conditions. Gels were stained and dried for autoradiography. The
distribution of PHGPx was calculated from scanning densitometry with a
Bio-Imaging Analyzer (BAS2000; Fuji Film, Tokyo).
Quantitation of Proteins--
Concentrations of protein were
determined with the BCA protein assay reagent (Pierce) with bovine
serum albumin as the standard.
Statistical Analysis--
All data for which n
3 are expressed as mean values ± S.D.
 |
RESULTS |
Expression of Selenoproteins and the Activities of Antioxidant
Enzymes in PHGPx-overexpressing RBL-2H3 Cells--
The distribution of
selenoproteins was determined in RBL-2H3 cells that had been labeled
with [75Se]sodium selenite for 4 days. Fig.
1 shows the electrophoretic profiles of
75Se-labeled proteins from control cells and
PHGPx-overexpressing RBL-2H3 cells. Three major selenoproteins were
detected, with estimated molecular masses of 57, 25, and 14 kDa
respectively. The band of a 20-kDa protein that corresponded to PHGPx
was quite faint in the control cells. The selenoproteins of 20 and 25 kDa were identified as cGPx and PHGPx, respectively, by
immunoprecipitation with corresponding antibodies (data not shown).
These results indicate that the level of PHGPx was quite low in the
control lines of cells as compared with that of cGPx. PHGPx was
extensively expressed in all lines of cells transfected with the
cDNA for PHGPx, whereas the levels of expressions of the other
three major selenoproteins in PHGPx-overexpressing cells were similar
to those in the control lines of cells.

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Fig. 1.
Expression of selenoproteins in cell lines
that had been stably transfected with the PHGPx expression vector in a
comparison with the control line of RBL2H3 cells. Control lines of
cells that had been transfected with the expression vector without the insert (S1, S2, and S6) and
PHGPx-overexpressing cells had been transfected with the expression
vector that included cDNA for rat PHGPx (L9, L10, and
L28). Cells were metabolically labeled with 75Se
(0.14 mCi/ml) for 4 days. Then the 75Se-labeled cells were
sonicated, and 50 µg of protein were loaded in each lane for analysis
by SDS-PAGE (12.5% polyacrylamide) with subsequent autoradiography for
detection of the 75Se-labeled selenoproteins.
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The specific activities of antioxidant enzymes were determined in the
PHGPx-overexpressing cells and control lines of cells as shown in Table
I. The activity of PHGPx in the
PHGPx-overexpressing cells was three times that in the control lines of
cells. No significant differences in the respective activities of cGPx,
glutathione S-transferase, and catalase between the
PHGPx-overexpressing cells and the control lines of cells were
observed.
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Table I
The activity of PHGPx (nmol/min/mg), cGPx (nmol/min/mg), glutathione
S-transferase (units/mg), and catalase (units/mg) in the control lines
of cells and in PHGPx-overexpressing cells
Data are means ± S.D. of results of six experiments.
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Production of Leukotrienes in the PHGPx-overexpressing RBL-2H3
Cells--
Levels of leukotrienes were determined in the control and
PHGPx-overexpressing cells after exposure to A23187 for 10 min by enzyme immunosorbent assays (Fig. 2).
Stimulated RBL-2H3 cells predominantly produced leukotriene
C4 (LTC4) and leukotriene B4 (LTB4), which reached levels of 2 and 0.2 ng/107 cells, respectively (Fig. 2A).
Overexpression of PHGPx in RBL2H3 cells led to a dramatic decrease in
the production of leukotrienes (Fig. 2B). Levels of both
leukotrienes produced in PHGPx-overexpressing cells were approximately
8 times lower than those in the control line of cells.

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Fig. 2.
Production of leukotrienes C4 and
B4 in control lines of cells and PHGPx-overexpressing
cells. Control lines of cells (A) and
PHGPx-overexpressing cells (B) were stimulated with 5 µM A23187 for 5 min at 37 °C. The amounts of
LTC4 (open bars) and LTB4
(hatched bars) were determined in the control cells
(S1, S2, and S6) and in the PHGPx-overexpressing
cells (L9, L10, and L28) by EIA. Values given are
means ± S.D. of results from three independent experiments.
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We examined the effects of diethyl malate (DEM) on the production of
leukotrienes to estimate whether or not the suppression of leukotriene
production had resulted from overexpression of PHGPx activity (Table
II). DEM inhibits the activity of
glutathione-dependent peroxidases, such as cGPx and PHGPx,
by lowering the level of glutathione in the cells. DEM caused a
decrease in the level of glutathione to about 2% that in non-treated
RBL-2H3 cells under the present conditions (data not shown). The
formation of leukotrienes was monitored in the control line of cells
and in PHGPx-overexpressing cells that had been pretreated with DEM for
3 h. The activity of cGPx, which was extensively expressed in the
control line of cells, was significantly suppressed by DEM under our
assay conditions. However, the total amounts of LTC4 and
LTB4 in the control line of cells were not altered in the
case of DEM-treated control cells even though the activity of cGPx was
significantly depressed. These results indicate that cGPx is not
involved in the regulation of leukotriene production. In contrast to
those in the control line of cells, rates of formation of
LTC4 and LTB4 were dramatically enhanced in
PHGPx-overexpressing cells after treatment with DEM. The production of
leukotrienes recovered to 80% that in the control line of cells after
inhibition of PHGPx activity by DEM. These results indicate that the
induction of PHGPx activity led to a reduction in the rate of
production of leukotrienes in RBL-2H3 cells.
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Table II
Effects of diethyl malate on the production of leukotrienes in a
control lines of cells and PHGPx-overexpressing cells
Control cells (S2) and PHGPx-overexpressing cells (L28) were
preincubated for 3 h at 37 °C with (+) or without ( ) 0.5 mM diethyl malate (DEM) for 3 h at 37 °C and then
stimulated with 5 µM A23187 for 5 min at 37 °C.
LTC4 and LTB4 (pg/107 cells), released into the
supernatant, were quantitated by EIAs. Values are given as means ± S.D. of results from three independent experiments.
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Depletion of glutathione also inhibits LTC4 synthetase,
which catalyzes the synthesis of LTC4 via the addition of
glutathione to LTA4. The rate of formation of
LTC4 was significantly reduced in the control cells by
treatment with DEM, and the accumulated LTA4 was
preferentially utilized for the synthesis of LTB4 by LTA4 hydrolase. The amount of LTB4 in
DEM-treated control cells was approximately 7 times that in non-treated
control cells, in which the production of LTC4 was markedly
inhibited by the treatment with DEM (Table II).
Inhibition of 5-Lipoxygenase Activity in PHGPx-overexpressing
Cells--
The rates of production of individual metabolites in the
5-lipoxygenase pathway, such as free arachidonic acid, 5-HETE,
LTC4, and LTB4, were determined in control line
of cells and in PHGPx-overexpressing cells that had been prelabeled
with [14C]arachidonic acid to determine the step at which
inhibition occurs in the 5-lipoxygenase pathway in PHGPx-overexpressing
cells (Fig. 3 and
4). A23187 induced the activation of
phospholipase A2 and provoked the liberation of free
arachidonic acid from membrane phospholipids (Fig. 3A). No
significant difference in the release of arachidonic acid was observed
between the control line of cells and the PHGPx-overexpressing cells.
Levels of cytosolic phospholipase A2
(cPLA2) were determined by immunoblot analysis with
anti-cPLA2 (Fig. 3B). The levels of
cPLA2 in PHGPx-overexpressing cells were almost the same as
that in the control line of cells. The rates of formation of 5-HETE,
LTC4, and LTB4 originated from
[14C]arachidonic acid were determined by reverse-phase
HPLC (Fig. 4). Peaks I and II contained LTC4 and
LTB4, respectively. Peak III contained 5-HETE that had been
produced by the reduction of 5-HPETE. The formation of three
5-lipoxygenase metabolites was facilitated in the control line of cells
after the challenge with A23187. By contrast, the rate of formation of
LTC4 and LTB4 from radioactive arachidonic acid
was significantly reduced in the PHGPx-overexpressing cells. The rate
of production of 5-HETE, formed by the reduction of 5-HPETE, was also
reduced in the PHGPx-overexpressing cells, although the capacity for
the reduction of 5-HPETE to 5-HETE was clearly elevated in the
PHGPx-overexpressing cells. Immunoblot analysis with anti
5-lipoxygenase and 5-lipoxygenase activating protein (FLAP) revealed
that levels of 5-lipoxygenase and FLAP were the same in
PHGPx-overexpressing cells and in the control line of cells (Fig.
5B). These results indicated
that activity of 5-lipoxygenase was inhibited in the
PHGPx-overexpressing cells and, as a result, the production of 5-HPETE,
the common precursor of LTC4, LTB4 and 5-HETE,
was significantly suppressed.

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Fig. 3.
Release of arachidonic acid and cellular
levels of cPLA2 in a control line of cells and in
PHGPx-overexpressing cells. A, release of arachidonic acid
from RBL-2H3 cells stimulated with A23187. Control line of cells (S2;
open bars) and PHGPx-overexpressing cells (L28; closed
bars) were prelabeled with [14C]arachidonic acid and
then stimulated with 5 µM A23187 for 10 min. The
radioactivity of free arachidonic acid in the supernatant was
determined. Values are means ± S.D. of results from five
independent experiments. B, detection of cPLA2
by immunoblot analysis. Cell lysates (50 µg of protein) of S2 cells
and L28 cells were subjected to SDS-PAGE and then proteins were blotted
onto a PVDF membrane. Immunoblotting was performed using polyclonal
antibodies against cPLA2 as described in the text.
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Fig. 4.
Separation by reverse-phase HPLC of
metabolites of 5-lipoxygenase produced by control line of cells and by
PHGPx-overexpressing cells after stimulation with A23187. A,
chromatographic profile of 5-lipoxygenase metabolites. The control line
of cells (S2; hatched bars) and PHGPx-overexpressing cells
(L28; closed bars) were prelabeled with
[14C]arachidonic acid and then stimulated with 5 µM A23187 for 10 min. The metabolites in supernatants and
cells were extracted with ethyl acetate and fractionated by
reverse-phase HPLC. The eluted fractions were collected for the
determination of radioactivity. Values given are as means ± S.D.
from five independent experiments. I, LTC4; II,
LTB4; III, 5-HETE. B, detection of 5-lipoxygenase and FLAP by immunoblot analysis. Lysates (50 µg of protein) for 5-lipoxygenase and nuclear fraction (50 µg of protein) for FLAP of
control line of cells (S2) and PHGPx-overexpressing cells
(L28) were subjected to SDS-PAGE and then proteins were
blotted onto a PVDF membrane. Immunoblotting was performed with
polyclonal antibodies against 5-lipoxygenase and FLAP, respectively, as
described in the text.
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Fig. 5.
Effects of 12-HPETE on the production of
LTC4. The control line of cells (A, S2) and
PHGPx-overexpressing cells (B, L28) were stimulated with 5 µM A23187 for 10 min after preincubation with various
amounts of 12-HPETE (hatched bars and closed
bars) or 12-HETE (open bars) for 10 min. Then levels of
LTC4 in supernatants were determined by EIA. Values
given are means ± S.D. of results from three independent
experiments.
|
|
To determine the effects of PHGPx on the activities of LTC4
synthase and LTA4 hydrolase, the PHGPx-overexpressing cells
and control lines of cells were incubated with 1 µM
exogenous LTA4 for 10 min. The productions of
LTC4 in the PHGPx-overexpressing cells (107
cells) and control lines of cells (107 cells) were 46 ± 5 and 50 ± 3 ng, respectively. The productions of
LTB4 in the PHGPx-overexpressing cells were almost same as that in the control lines of cells accounting for approximately 8 ng/107 cells. These results indicate that no significant
differences of activities of LTC4 synthase and
LTA4 hydrolase were observed in the PHGPx-overexpressing
cells and the control lines of cells.
Involvement of HPETE in the Suppression of 5-Lipoxygenase Activity
in PHGPx-overexpressing Cells--
We determined the effects of
hydroperoxides on the production of leukotrienes in an attempt to
estimate whether the inhibition of the activity of 5-lipoxygenase was
due to insufficient levels of hydroperoxides in PHGPx-overexpressing
cells (Fig. 5). Levels of LTC4 in A23187-stimulated cells
were determined in the presence of various concentrations of 12-HPETE,
which is not utilized as a substrate for the synthesis of
LTC4. The rate of formation of LTC4 in the
PHGPx-overexpressing cells was significantly increased by the addition
of 12-HPETE, and it returned to the rate in the control line of cells
at a concentration of 12-HPETE of 5 ng (Fig. 5B). By
contrast, 12-HPETE had no effect in the control line of cells (Fig.
5A). 12-HETE, a reduced form of 12-HPETE, failed to restore
the production of LTC4 in PHGPx-overexpressing cells.
The levels of hydroperoxides were determined in the control line of
cells and in the PHGPx-overexpressing cells by flow cytometric analysis
after incorporation by cells of 2
,7-dichlorofluorescein diacetate
(DCFH-DA), a hydroperoxide-sensitive fluorescent dye (Fig.
6). The basal fluorescence intensity of
DCFH in PHGPx-overexpressing cells was lower than that observed in the
control line of cells (Fig. 6A). A23187 provoked the
production of intracellular hydroperoxides, and the intensities of
peaks of fluorescence increased. The increase in fluorescence intensity
in A23187-stimulated control cells was larger than that in similarly
stimulated PHGPx-overexpressing cells (Fig. 6B). These
results indicate that the levels of hydroperoxides in
PHGPx-overexpressing cells were much lower than those in the control
line of cells without stimulation and also after stimulation with
A23187. The levels of hydroperoxide in PHGPx-overexpressing cells after
the addition to the medium of 10 ng of 12-HPETE were the same as the
basal level in the control line of cells (Fig. 6C). The
intensity of fluorescence after stimulation with A23187 of
PHGPx-overexpressing cells that had been pretreated with 12-HPETE was
the same as that in the control line of cells after stimulation with
A23187 (Fig. 6D). These results indicated that the increase in levels of intracellular hydroperoxides, caused by the addition of
12-HPETE, in PHGPx-overexpressing cells had dramatically increased the
rate of formation of intracellular hydroperoxides.

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Fig. 6.
Detection of intracellular hydroperoxides by
flow cytometric analysis. The control line of cells (S2) and
PHGPx-overexpressing cells (L28) were preincubated with 10 ng of
12-HPETE (C and D) or without 12-HPETE
(A and B) for 10 min at 37 °C and then they were stimulated with 5 µM A23187 (B and
D) or not stimulated (A and C) for 10 min. Flow cytometric analysis of cells was performed using DCFH-DA. The
intensity of fluorescence of DCFH was plotted, on a logarithmic scale
in arbitrary units, against the number of control cells (white
areas) and the number of PHGPx-overexpressing cells (black
areas), respectively.
|
|
Subcellular Localization of PHGPx in PHGPx-overexpressing
Cells--
To investigate the amounts of PHGPx in nuclear fraction of
the control line of cells and PHGPx-overexpressing cells, cells prelabeled with [75Se]sodium selenite for 4 days were
fractionated into their organelle by the centrifugation, solubilized,
and immunoprecipitated with anti-PHGPx. PHGPx was mainly enriched both
in the mitochondrial and the nuclear fraction in the control line of
cells (Fig. 7, A and
C). In PHGPx-overexpressing cells, the amounts of PHGPx were
significantly enhanced in nuclear, microsomal, and cytosolic fractions
(Fig. 7, B and D). The amount of PHGPx associated
with nuclear fractions from PHGPx-overexpressing cells was 3.5 times higher than that from the control line of cells (C and
D).

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Fig. 7.
Subcellular localization of PHGPx in the
control line of cells and PHGPx-overexpressing cells. The control
line of cells (S2: A and C) and
PHGPx-overexpressing cells (L28: B and D) were
metabolically labeled with 75Se (0.14 mCi/ml) for 4 days.
The 75Se-labeled cells were fractionated by differential
centrifugation into nuclear fraction (N), mitochondrial
fraction (M), microsomal fraction (Mc), and
cytosolic fraction (S). The distributions of marker proteins
in individual subfractionation were determined by enzymatic activity
and immunoblot analysis (A and B). Lactate dehydrogenase (LDH), cytochrome c oxidase
(Cyt Ox), and NADPH-cytochrome c reductase
(Cyt Red) were measured as marker enzymes of cytosol, mitochondria, and microsome, respectively. Distribution of histone H1
(Histon) as marker protein of nucleus was calculated from
scanning densitometry by a Bio-Imaging Analyzer as described in the
text. Distribution of PHGPx was determined by immunoprecipitation
analysis with anti-PHGPx (C and D). Relative
radioactivity of PHGPx was calculated from scanning densitometry by a
Bio-Imaging Analyzer.
|
|
 |
DISCUSSION |
RBL-2H3 cells have a potent 5-lipoxygenase activity and are
popular model cells for the studies of the production of
leukotrienes (29, 30). The present study demonstrated that the
overexpression of PHGPx in RBL2H3 cells caused a dramatic suppression
of the production of leukotrienes in response to stimulation by A23187 (Fig. 2). The production of individual metabolites of 5-lipoxygenase was examined in PHGPx-overexpressing cells that had been preincubated with [14C]arachidonic acid by reverse-phase HPLC to
define the step in the 5-lipoxygenase pathway where inhibition occurs
(Fig. 4A). The rates of production of radioactive 5-HETE,
LTC4, and LTB4 in PHGPx-overexpressing cells
were much lower than in the control line of cells, whereas the rates of
release of [14C]arachidonic acid were unchanged (Fig. 3).
No esterification of 5-HETE in phospholipid was also detected in
PHGPx-overexpressing cells (data not shown). Suppression of the
production of 5-HETE in PHGPx-overexpressing cells indicated that
inhibition of the synthesis of leukotrienes was not due to acceleration
of the reduction of 5-HPETE to 5-HETE but was, rather, due to the
inhibition of the production of 5-HPETE from arachidonic acid by
5-lipoxygenase. Levels of 5-lipoxygenase did not change in
PHGPx-overexpressing cells (Fig. 4B), an indication that the
activity of 5-lipoxygenase was suppressed in such cells.
The question remains as to how PHGPx down-regulates the activity of
5-lipoxygenase. The results obtained with PHGPx-overexpressing cells
clearly indicate that PHGPx is intimately involved in the suppression
of the activity of 5-lipoxygenase. Previous reports suggest that lipid
hydroperoxides have dual effects on the activity of 5-lipoxygenase. In
studies of enzyme kinetics, a small amount of HPETE activated
5-lipoxygenase (48), and a relatively high concentration (1.75 µM) of HPETE caused inactivation (49). Although the
precise mechanisms of the activation and inactivation of 5-lipoxygenase have not been elucidated, it seems likely that the state of the iron in
5-lipoxygenase might modulate the activity of the enzyme. When
lipoxygenase is inactive, the enzyme contains a single non-heme iron
that is in the ferrous oxidation state (Fe2+). The active
form of lipoxygenase contains iron in the ferric oxidation state
(Fe3+) (50, 51). Thus, the conversion of iron to the ferric
from the ferrous oxidation state is necessary for the activation of lipoxygenase (52-55). Therefore, the activity of lipoxygenase might be
regulated by a small amount of hydroperoxy lipids, acting as essential
activators of the enzyme. In the present study, preincubation of
PHGPx-overexpressing cells with 12-HPETE led to increased production of
leukotrienes, whereas 12-HPETE did not affect the production of
leukotrienes in the control line of cells (Fig. 5). Our results indicate that PHGPx is primarily responsible for the reduction of lipid
hydroperoxides and thereby cause the down-regulation of 5-lipoxygenase
in RBL-2H3 cells.
Flow cytometric analysis revealed that the basal level of intracellular
hydroperoxides was significantly reduced in PHGPx-overexpressing cells
(Fig. 6). A rapid and transient increase in levels of intracellular hydroperoxides induced by stimulation with A23187 was observed. The
increase in fluorescence intensity was probably due to the production
of intracellular lipid hydroperoxides, including 5-HPETE produced by
5-lipoxygenase. The increase in the levels of intracellular lipid
hydroperoxides induced by A23187 was suppressed by overexpression of
PHGPx. This effect by PHGPx was abolished by the addition of a small
amount of 12-HPETE, which probably restored the production of
LTC4. Thus, small variations in the levels of intracellular hydroperoxides can dramatically modulate the production of
leukotrienes, and PHGPx seems to be able to regulate the activity of
5-lipoxygenase by modulating the levels of intracellular lipid
hydroperoxides.
It is assumed that levels of lipid hydroperoxides are controlled by two
kinds of intracellular GPx isozyme. Previous studies suggested that GPx
might modulate the activity of 5-lipoxygenase because depletors of
glutathione such as 1-chloro-2,4-dinitrobenzene or diamide induce the
enhanced production of leukotrienes in human polymorphonuclear
leukocytes (24) and B lymphocytes (22, 23). To evaluate whether it is
cGPx or PHGPx that has such an effect, we examined the effects of an
inhibitor of GPx on the production of leukotrienes in the control line
of cells and in PHGPx-overexpressing cells (Table II). The production
of LTC4 and LTB4 in the control line of cells
was not influenced by the treatment with DEM, even though the activity
of cGPx, as the predominant GPx in the control line of cells, was
inhibited by the depletion of glutathione. By contrast, the production
of leukotrienes was significantly increased in the PHGPx-overexpressing
cells when PHGPx activity was inhibited by DEM. These results indicate
that PHGPx was involved in the inhibition of the activity of
5-lipoxygenase, whereas cGPx did not affect this activity.
PHGPx is located in the cytosol and membrane fraction, and cGPx is
known to be present predominantly in the cytosol. Godeas et
al. (56) demonstrated the specific localization of PHGPx in
nuclear and mitochondrial fractions of rat testis. PHGPx has the
highest ability to reduce lipid hydroperoxides in membranes of the four
known isozymes of GPx (57). We showed subcellular localization of PHGPx
in the control line of cells and PHGPx-overexpressing cells (Fig. 7).
Control line of RBL2H3 cells contained the small amounts of PHGPx in
the cytosol, whereas the large amounts of PHGPx are localized in the
mitochondria and nucleus. In PHGPx-overexpressing cells, the amounts of
PHGPx were significantly enhanced in nuclear, microsomal, and cytosolic
fractions. The amount of PHGPx in nuclear fractions from
PHGPx-overexpressing cells was 3.5 times higher than that from the
control line of cells (Fig. 7). The synthesis of leukotrienes occurs at
the nuclear membrane where cytosolic phospholipase A2 and
5-lipoxygenase have been translocated from the cytosol (6, 7). The
expression of PHGPx in the nucleus might be critical for modulation of
the trace amounts of lipid hydroperoxide required for the activation of
5-lipoxygenase. Overexpression of PHGPx did not affect the
translocation of 5-lipoxygenase and cytosolic phospholipase
A2 from the cytosol to the nucleus in RBL-2H3 cells (data
not shown). These results indicate that inactivation of
5-lipoxygenase was due to high level expression of PHGPx in the
nucleus.
Metabolites of arachidonic acid seem to play an important physiological
role in the signal transduction system that includes activation of
NF
B (58) and AP-1 (59), as well as in the regulation of cell
survival and apoptosis (60, 61). Furthermore, LTB4 is not
only a powerful chemotactic factor through LTB4 receptor in
inflammation (62) but is also an activator of the transcription factor
PPAR
(the peroxisome proliferator-activated receptor
) (63).
Thus, metabolites of lipoxygenase have a variety of biological activities in addition to their functions as chemical mediators. The
present study suggests that PHGPx might be involved in the regulation
of cellular functions and signal transduction through modulation of the
production of leukotrienes.
 |
ACKNOWLEDGEMENTS |
We thank Kae Iwasaki and Miyuki Naito for
their expert technical assistance. We also thank the Kitasato Institute
for help with the flow cytometric analysis.
 |
FOOTNOTES |
*
This work was supported in part by Grant-in-Aid 07772179 from the Ministry of Education, Science and Culture of Japan, a grant from the Fujisawa Foundation, and a grant from the Japan Health Science
Foundation.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: School of
Pharmaceutical Sciences, Kitasato University, 5-9-1 Shirokane,
Minato-ku, Tokyo 108, Japan. Tel. and Fax: 81-3-3444-4943; E-mail:
nakagaway{at}pharm.kitasato-u.ac.jp.
1
The abbreviations used are: HPETE,
hydroperoxyeicosatetraenoic acid; cGPx, cytosolic glutathione
peroxidase; cPLA2, cytosolic phospholipase A2;
DCFH-DA, 5,6-carboxy-2
,7
-dichlorofluorescein-diacetate; DEM, diethyl
malate; EIA, enzyme immunosorbent assay; FLAP,
5-lipoxygenase-activating protein; GSH, glutathione; HETE,
hydroxyeicosatetraenoic acid; HPLC, high performance liquid
chromatography; LT, leukotriene; PBS, phosphate-buffered saline; PCOOH,
phosphatidylcholine hydroperoxide; PHGPx, phospholipid hydroperoxide
glutathione peroxidase; GPx, glutathione peroxidase; PMSF,
phenylmethylsulfonyl fluoride; PVDF, polyvinylidene difluoride; PAGE,
polyacrylamide gel electrophoresis.
 |
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