Potential Role for Ceramide in Mitogen-activated Protein Kinase Activation and Proliferation of Vascular Smooth Muscle Cells Induced by Oxidized Low Density Lipoprotein*

Nathalie AugéDagger §, Isabelle Escargueil-BlancDagger §parallel , Isabelle Lajoie-MazencDagger **, Isabelle SucDagger , Nathalie Andrieu-AbadieDagger , Marie-Thérèse PieraggiDagger , Martine ChatelutDagger , Jean-Claude ThiersDagger , Jean-Pierre JaffrézouDagger Dagger , Guy LaurentDagger Dagger , Thierry LevadeDagger , Anne Nègre-SalvayreDagger §§, and Robert SalvayreDagger §§

From the Dagger  Laboratory of Biochemistry, INSERM U-466, Institut Louis Bugnard, CHU Rangueil, 1 Avenue Jean Poulhes, 31403 Toulouse Cedex 4, France and Dagger Dagger  INSERM CJF-9503, Centre Claudius Regaud, 20 Rue du Pont Saint-Pierre, 31052 Toulouse Cedex, France

    ABSTRACT
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Proliferation of vascular smooth muscle cells (SMC) is a hallmark in the pathogenesis of atherosclerotic lesions. Mildly oxidized low density lipoproteins (UV-oxLDL), which are mitogenic to cultured AG-08133A SMC, activate the sphingomyelin (SM)-ceramide pathway. We report here the following. (i) UV-oxLDL elicited a biphasic and sustained activation of MBP kinase activity, phosphorylation and nuclear translocation of p44/42 mitogen-activated protein kinase (MAPK), and [3H]thymidine incorporation, which were inhibited by PD-098059, a MAPK kinase inhibitor. (ii) The use of preconditioned media (from SMC pre-activated by UV-oxLDL) transferred to native SMC and blocking antibodies against growth factors suggest that UV-oxLDL-induced activation of MAPK and [3H]thymidine incorporation seem to be independent of any autocrine secretion of growth factors. (iii) UV-oxLDL-induced activation of a neutral sphingomyelinase, SM hydrolysis, ceramide production, and [3H]thymidine incorporation were inhibited by two serine-protease inhibitors (serpins), suggesting that a serpin-sensitive proteolytic pathway is involved in the activation of the SM-ceramide signaling pathway. (iv) UV-oxLDL-induced MAPK activation and [3H]thymidine incorporation were mimicked by ceramide generated in the plasma membrane by bacterial sphingomyelinase treatment or by addition of the permeant C2-ceramide. Serpins did not inhibit the MAPK activation and [3H]thymidine incorporation induced by C2-ceramide, indicating that activation of the MAPK and [3H]thymidine incorporation is subsequent to the stimulation of the SM-ceramide pathway. Taken together, these data suggest that mitogenic concentrations of UV-oxLDL are able to stimulate the SM-ceramide pathway through a protease-dependent mechanism and activate p44/42 MAPK, leading to proliferation of vascular SMC.

    INTRODUCTION
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Atherosclerosis, and its complications, namely myocardial infarction, stroke, and peripheral vascular diseases, is one of the most prevalent cause of morbidity and mortality in Western countries. During atherogenesis, focal lesions spread out progressively and lead to the formation of fibro-atheroma plaques, in which smooth muscle cell (SMC)1 proliferation plays a critical role (1, 2). Among the risk factors identified, low density lipoprotein (LDL) cholesterol level is strongly predictive of coronary heart disease. LDL are believed to have an important role in atherogenesis (3), following oxidative modifications (4-6), because oxidized LDL are present in atherosclerotic lesions (7) and possess a wide range of biological properties potentially occurring during atherogenesis in vivo (8). Oxidized LDL have recently been shown to be mitogenic to vascular SMC (9-11). These studies suggest that oxidized LDL may be considered as an additional mitogenic factor, alongside the classical growth factors implicated in SMC proliferation during atherogenesis (6). To date, the mechanism of the oxidized LDL proliferative effect is poorly elucidated and may result from the triggering of a mitogenic intracellular signal either directly by oxidized LDL or indirectly through an autocrine effect involving growth factor secretion and/or growth factor receptor over-expression.

Recently, sphingolipids have emerged as key signaling molecules involved in the regulation of cell growth and differentiation (for reviews, see Refs. 12-15). In particular, the sphingomyelin (SM; ceramide phosphocholine)-ceramide pathway appears as a prototypic sphingolipid signaling pathway implicated in the positive or negative regulation of cell growth. Activation of this pathway leads to SM hydrolysis and subsequent generation of ceramide, the backbone of all sphingolipids, which serves as an intracellular second messenger. To date, several agents have been described to stimulate the SM-ceramide pathway (reviewed in Refs. 12 and 14-17), including cytokines such as TNFalpha , interleukin-1beta , interferon gamma , nerve growth factor, anti-CD28, anti-Fas antibodies, anticancer drugs, and ionizing radiations (18-21). Cell-permeant ceramides, or ceramide produced by treatment of intact cells with exogenous sphingomyelinase, can mimic the effects of various inducers of the SM-ceramide pathway. Thus, various cellular responses including cell proliferation (18), differentiation (22), or apoptosis (19, 20, 23) seem to be transduced by SM hydrolysis through ceramide generation. We have recently reported that the SM-ceramide pathway is involved in the mitogenic signaling triggered by mildly oxidized LDL (UV-oxLDL) in SMC (11).

Cell proliferation promoted by extracellular growth stimuli involves various intracellular signaling pathways leading to activation of gene transcription, DNA synthesis, and cell division (24, 25). Protein phosphorylation, mediated by a complex regulatory network of protein kinases, plays an essential role in the signal transduction between cell surface and nucleus (26). Despite the broad diversity of mitogens and receptors, these signaling pathways often converge toward the mitogen-activated protein (MAP) kinases, a group of serine/threonine protein kinases also referred to as extracellular-regulated kinases (ERKs; p44/ERK1 and p42/ERK2, p44/42 MAPK) in mammalian cells (26). MAPKs are rapidly activated in response to stimulation of receptors for growth factors, hormones, or cytokines, G protein-coupled receptors, or in response to stress (25, 27-29). They are activated by phosphorylation on both Tyr and Thr residues (30) by the dual specificity MAPK kinases, which are activated by Raf (29). The activation of MAPKs, associated with their nuclear translocation, is essential to trigger entry into the S phase of cell cycle (31, 32).

The data reported in this study suggest that mitogenic concentrations of UV-oxLDL elicit the activation of the SM-ceramide pathway through a protease-dependent process. Subsequently, it induced a sustained activation and nuclear translocation of p44/42 MAPK and [3H]thymidine incorporation in cultured vascular SMC.

    EXPERIMENTAL PROCEDURES
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Chemicals-- [3H]Thymidine (5 Ci/mmol) and horseradish peroxidase-conjugated sheep anti-mouse Ig were obtained from Amersham (Les Ulis, France). [gamma -32P]ATP (7000 Ci/mmol) was from ICN (Orsay, France), [gamma -33P]ATP (5 Ci/mmol) was from Isotopchim (Ganagobie, France), [methyl-3H]choline chloride (86 Ci/mmol), [choline-methyl-14C]SM (54.5 mCi/mmol), and [9,10-3H]palmitic acid (52 Ci/mmol) were from DuPont NEN (Les Ulis, France). Human recombinant growth factors (PDGF, bFGF, and EGF) were obtained from PeproTech-Tebu (Le Perray, France). Antibodies, anti-PDGF (goat polyclonal), anti-bFGF (mouse monoclonal), and anti-EGF (rabbit polyclonal), anti-phosphotyrosine (4G10, mouse monoclonal) were purchased from Euromedex (Souffelweyersheim, France); rabbit polyclonal anti-ERK1 and anti-ERK2 (C-16 and CK-23) was purchased from Santa Cruz Biotechnologies (Santa Cruz, CA), horseradish peroxidase-conjugated goat anti-rabbit IgG was purchased from Bio-Rad (Ivry, France), and fluorescein isothiocyanate-conjugated anti-rabbit IgG was purchased from BioSys (Compiègne, France). Acrylamide bisacrylamide was from Bioprobe (Montreuil-sous-Bois, France), nitrocellulose membranes and protein A-Sepharose were from Pharmacia (St Quentin-en-Yvelines, France), and DiIC18 (1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbo-cyanine perchlorate) was from Molecular Probes. N-Tosyl-L-phenylalanyl chloromethyl ketone (TPCK), dichloroisocoumarin (DCIC), C2-ceramide, and Bacillus cereus sphingomyelinase were purchased from Sigma, and DHC (C2-dihydroceramide or N-acetylsphinganine) was from Biomol/Tebu (Le Perray, France). Inhibitors were generally dissolved in ethanol and administered to the cells at a final concentration <0.1%. B. cereus phospholipase C was supplied by Boehringer Mannhein (Meylan, France). RPMI 1640 medium containing 2 mM Glutamax, fetal calf serum (FCS), and antibiotics were from Life Technologies, Inc. (Cergy-Pontoise, France). Other chemicals were obtained from Sigma or Merck.

Cell Culture-- Bovine aortic SMC (AG-08133A, from the NIA Aging Cells Repository, Camden, NJ) were grown in RPMI 1640 medium supplemented with 10% FCS, penicillin (100 units/ml), and streptomycin (100 µg/ml), at 37 °C in humidified 5% CO2. After trypsinization, cells were grown in medium containing 10% FCS for 24 h. Then, the medium was removed, and cells were washed once with RPMI and grown for 48 h in RPMI medium containing 1% FCS prior to the addition of native or oxidized LDL. In some experiments, SV40-transfected SMC cells were used. For this purpose, SMC were electroporated (240 V, 960 µF) with a plasmid (pAS) carrying the large T antigen (33); these transfected SMC exhibited a two to three times longer life span than the untransfected cells. For the experiments presented here, similar results were obtained with either SMC type.

Lipoprotein Isolation and Oxidation by UV-C-- Human LDL (d 1.019-1.063) were isolated from pooled fresh sera by sequential ultracentrifugation, dialyzed, sterilized by filtration, and stored at 4 °C under nitrogen until use, as described previously (10). Mildly oxidized LDL (UV-oxLDL) were prepared by UV-C irradiation under the previously defined standard conditions (254 nm, 0.5 mW/cm2 for 2 h) (34).

Labeling of LDL with DiIC18 and Determination of LDL Uptake by SMC-- Purified LDL were fluorescently labeled with DiIC18 according to Via and Smith (35), re-isolated by ultracentrifugation, and dialyzed and sterilized again as indicated above. DiIC18-labeled LDL were added to the culture medium (100 µg of apoB/ml) and incubated with cells for the indicated times. Then, cells were washed once with PBS containing 5 g/liter bovine serum albumin and twice with PBS only. Afterward, cells were homogenized by sonication in 1 ml of distilled water, and an aliquot was used to extract DiIC18 by the procedure of Folch et al. (36) and to read the cell-associated fluorescence extracted in the chloroformic phase (using a Jobin-Yvon JY-3C spectrofluorometer; excitation 545 nm, emission 568 nm).

[3H]Thymidine Incorporation Assays-- DNA synthesis was evaluated by [3H]thymidine incorporation (at time 24 h, under standard conditions, or at the time indicated in the figures). Cells (2 × 105/dish) were labeled for 12 h with [3H]thymidine (0.5 µCi/ml) before harvesting and then washed three times with PBS; after addition of 3% perchloric acid, the acid-precipitable material was dissolved overnight in 1 N NaOH, 1% SDS and counted by liquid scintillation (Packard Tricarb 4530 counter).

Quantitation of Sphingolipids and Sphingomyelinase Assays-- SMC were metabolically labeled to equilibrium with [methyl-3H]choline (0.5 µCi/ml) or [3H]palmitic acid (0.5 µCi/ml) in RPMI medium containing 1% FCS. After 48 h of incubation, cells (about 300,000/assay) were washed once with PBS and chased for 2 h in fresh RPMI containing 1% FCS. Then, the medium was replaced by fresh 1% FCS-containing medium with or without UV-oxLDL (100 µg of apoB/ml). At the indicated times, cells were washed with ice-cold PBS, harvested using a rubber policeman, and sedimented by centrifugation (300 × g for 5 min). Cell pellets were immediately frozen at -20 °C. Cell pellets were suspended in 0.6 ml of distilled water and homogenized by sonication (2 × 10 s, using an MSE probe sonicator). An aliquot was saved for protein determination (37). Lipids from 0.5 ml of the cell lysate were extracted by 2.5 ml of chloroform/methanol (36), and [3H]choline-labeled SM and [3H]palmitoyl-labeled ceramide were quantified as described previously (11, 38).

Neutral and alkaline SMase activities were determined essentially as described by Wiegmann et al. (39) but in the presence or absence of EDTA under the previously used conditions (21). Briefly, cells were homogenized by sonication (2 runs of 10 s as above indicated) in 0.1% Triton X-100, 10 mM MgCl2, 5 mM dithiothreitol, 0.1 mM Na3VO4, 10 mM beta -glycerophosphate, 750 µM ATP, 1 mM PMSF, 2 mM EDTA, 10 µM leupeptin, and 10 µM pepstatin. SMase assays contained 100 µl of cell homogenate (100 µg of protein) and 100 µl of substrate [choline-methyl-14C]SM (120,000 dpm/assay) in 0.1% Triton X-100, 20 mM HEPES buffer, pH 7.4, containing 1 mM MgCl2 (and 10 mM EDTA when indicated) for the neutral activity, or in 250 mM Tris-HCl buffer, pH 8.5, containing 0.1% Triton X-100 for the alkaline activity. For determining acid SMase activity, cells were homogenized by sonication in 0.1% Triton X-100. Assays contained 100 µl of cell homogenate (100 µg of protein) and 100 µl of substrate [choline-methyl-14C]SM (120,000 dpm/assay) in 250 mM acetate buffer, pH 5.0, containing 0.1% Triton X-100. After 2 h of incubation at 37 °C, the liberated [methyl-14C]choline was partitioned by the Folch procedure (36) under the previously used conditions (21) and quantitated by liquid scintillation counting.

Measurement of MAP Kinase Activity-- MAP kinase activity was determined on immunoprecipitates according to a procedure derived from Ikeda et al. (40). Briefly, after incubation with (or without) LDL, cells (2 × 107) were placed on dry ice, washed twice with cold PBS, and scraped off with a rubber policeman in buffer A (20 mM Tris-HCl buffer, pH 7.4, containing 50 mM NaCl, 50 mM NaF, 5 mM EDTA, 20 mM sodium pyrophosphate, 1 mM Na3VO4, 100 µg/ml PMSF, 1 µg/ml leupeptin, and 1 µg/ml aprotinin). After centrifugation (300 × g for 10 min), the cell pellets were lysed for 30 min at 4 °C in 500 µl of lysis buffer B (20 mM Tris-HCl, pH 7.4, containing 10 g/liter Triton X-100, 1 g/liter SDS, 50 mM NaCl, 50 mM NaF, 5 mM EDTA, 20 mM sodium pyrophosphate, 1 mM Na3VO4, 100 µg/ml PMSF, 1 µg/ml leupeptin, and 1 µg/ml aprotinin). Samples were centrifuged (12,500 × g for 10 min, 4 °C). A 5-µl aliquot of the supernatant was used for protein determination (37). The supernatant was precleared for 1 h at 4 °C with 5 mg of protein A-Sepharose. After centrifugation (12,500 × g for 5 min), the supernatant was incubated for 4 h at 4 °C with 5 µl of anti-ERK1 antibody (100 µg/ml), and 5 mg of protein A-Sepharose was added for 1 h at 4 °C. After centrifugation (12,500 × g for 5 min), the pellet was washed twice with buffer A, solubilized in 200 µl of extraction buffer (20 mM Tris-HCl, pH 7.4, 60 mM glycerophosphate, 10 mM EGTA, 10 mM MgCl2, 0.1 mM NaF, 2 mM dithiothreitol, 1 mM Na3VO4, 20 mg/ml leupeptin, and 1 mM PMSF) and used for determining the MAP kinase activity by phosphorylation of MBP in the presence of [gamma -33P]ATP (300,000 dpm/assay) as described (40, 41). The reaction mixtures were spotted on phosphocellulose discs, which were washed with 10% cold trichloroacetic acid containing 10 mM sodium pyrophosphate. After drying, the discs were counted by liquid scintillation. Alternatively, proteins were separated by electrophoresis in a 10% polyacrylamide gel, and the radioactivity was visualized by autoradiography (Biomax-MR, Eastman Kodak).

Western Blotting-- Phosphotyrosine proteins were detected in SMC by Western blotting (42). Cells (2 × 106/assay) were solubilized in 100 µl in lysis buffer B for 30 min at 4 °C, centrifuged (12,500 × g for 10 min at 4 °C), and 100 µg of protein of the supernatant were subjected to SDS-polyacrylamide gel electrophoresis (100 V, 9 mA for 16 h). Proteins were transferred to nitrocellulose membranes (300 V, 200 mA for 5 h), blocked with 5% nonfat milk in Tris-buffered saline-Tween 20 (0.1%) at 4 °C for 2 h and incubated overnight at 4 °C with anti-phosphotyrosine 4G10 monoclonal antibody (dilution 1:500). The membranes were washed four times in Tris-buffered saline-Tween 20, and antibody reactions were detected using horseradish peroxidase-conjugated sheep anti-mouse IgG (dilution 1:3000) and the ECL chemiluminescent detection reagents (Amersham) according to the manufacturer's instructions. Alternatively, the cell lysate was precleared on protein A-Sepharose and immunoprecipitated with an anti-phosphotyrosine (PY20) monoclonal antibody exactly under the conditions described above for immunoprecipitating MAPKs with anti-ERK. Then, tyrosine-phosphorylated proteins, heated (90 °C for 10 min) and dissolved in the electrophoresis buffer, were resolved by SDS-polyacrylamide gel electrophoresis, transferred onto nitrocellulose membranes, and probed with anti-ERK1 or anti-ERK2 antibody, as indicated above.

Indirect Immunofluorescence-- SMC, grown on uncoated glass coverslips, were fixed in PBS and 3% paraformaldehyde for 15 min, permeabilized with 0.1% Triton X-100, and incubated with anti-ERK1 antibody (1:40) for 30 min. After washing three times with PBS, incubation with a secondary fluorescein isothiocyanate-conjugated anti-rabbit IgG for 30 min, and washing again with PBS, slides were mounted in Fluoprep and examined by fluorescence microscopy using a Diaplan (Leitz) or a confocal laser scanning microscope (Zeiss, LSM model).

    RESULTS
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MAPK Activation in AG-08133A SMC Treated by UV-oxLDL-- The UV-oxLDL used here were defined by moderate lipid peroxidation (4 ± 1 nmol of thio-barbituric acid-reactive substances/mg of apoB) and only minor modifications of apoB (as shown by minor alterations of the electrophoretic mobility, no significant loss of surface amino groups and cellular uptake through the apoB/E receptor) (34, 43). We utilized here a concentration of UV-oxLDL (100 µg of apoB/ml) that gave maximal mitogenic effect to cultured AG-08133A SMC (as shown by [3H]thymidine incorporation) and only a low level of cytotoxicity, as assessed by LDH release (10, 11).

Mitogenic concentrations of UV-oxLDL induced a biphasic increase of MBP kinase activity in SMC (Fig. 1, A and B). A first, transient peak of MAPK activity, maximal at 1 h, was followed by a second rise, sustained for at least 3 h. Native LDL induced a weak transient peak but not the second sustained peak of MBP kinase (Fig. 1, A and B). Similar results were obtained when using whole cell extracts (Fig. 1A) and anti-ERK immunoprecipitates (data not shown). To provide more evidence for the MAPK activation in SMC stimulated by mitogenic doses of UV-oxLDL, tyrosine phosphorylation of MAPK was examined by immunoblotting. As reported in Fig. 1C, UV-oxLDL induced an increase of tyrosine phosphorylation of p44 and p42 that was evident after 1 h of incubation and plateaued at 3-5 h. As shown in Table I, both the MAPK activation (peaks at 1 and 3 h) and the proliferative effect induced by UV-oxLDL were inhibited by 10 µM PD-098059, a MAPK kinase inhibitor (44). This suggests the involvement of the MAPK cascade in the mitogenic signaling triggered by UV-oxLDL.


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Fig. 1.   Activation of MAPK by UV-oxLDL in cultured AG-08133A SMC. A, time course of MBP kinase activation in response to UV-oxLDL (filled symbols) or native LDL (empty symbols). SMC were starved in RPMI containing 1% FCS for 48 h before the contact with LDL. Then, cells were incubated with UV-oxLDL or native LDL (100 µg of apoB/ml). MBP kinase activity was determined after immunoprecipitation of MAPK using anti-ERK1/ERK2, as described under "Experimental Procedures." Mean ± S.E. of three separate experiments. B, autoradiography showing the time course of MBP phosphorylation. SMC were treated under the conditions of A with 100 µg of apoB/ml of UV-oxLDL or native LDL (upper and lower panels, respectively), and assays for MBP phosphorylation were performed under the conditions described under "Experimental Procedures." C, tyrosine phosphorylation of MAPK. SMC were incubated with UV-oxLDL or native LDL (100 µg of apoB/ml) for the indicated times. SMC lysates were immunoprecipitated with anti-phosphotyrosine protein antibody, resolved on SDS-polyacrylamide gel electrophoresis, and revealed with anti-ERK1/ERK2 antibody.

                              
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Table I
Effect of PD-098059, a MAPK kinase inhibitor, and RNA and protein synthesis inhibitors on MAPK activation and proliferation of AG-08133A SMC induced by UV-oxLDL
Mean ± S.E.M. of three to four experiments.

Subsequently to mitogenic stimulation, activated MAPKs have been shown to be translocated into the nucleus (31, 45, 46). Therefore, we investigated, by immunofluorescence microscopy, the subcellular localization of MAPKs in SMC incubated with mitogenic doses of UV-oxLDL. As illustrated in Fig. 2, MAPKs underwent a nuclear translocation, which was maximal between 3 and 5 h after the beginning of the incubation of SMC with UV-oxLDL.


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Fig. 2.   Nuclear translocation of MAPK induced by UV-oxLDL in AG-08133A SMC. Cells were prepared under the conditions of Fig. 1 and were incubated for 3 h with (A and B) or without (C and D) UV-oxLDL (100 µg of apoB/ml). Cells were labeled by indirect immunofluorescence using anti-ERK1/ERK2 antibody and observed by fluorescence microscopy (A and C) or confocal laser fluorescence microscopy (B and D).

MAPK Activation and Proliferation Triggered by UV-oxLDL in AG-08133A SMC Do Not Result from an Autocrine Secretion of Growth Factors-- As oxidized LDL have been shown to enhance the expression of various growth factors (6), we investigated whether an autocrine mechanism (secretion of growth factors by AG-08133A SMC treated by UV-oxLDL) may be involved in the mitogenic signaling and the proliferative effect induced by oxidized LDL.

The effect of RNA and protein synthesis inhibitors on MAPK activation elicited by UV-oxLDL was investigated by preincubating the cells for 2 h with 50 nM actinomycin D or 10 µM cycloheximide just before addition of 100 µg of apoB/ml of UV-oxLDL. This treatment did not block the MAPK activation (neither the first transient nor the sustained peaks) induced by UV-oxLDL (Table I). This suggests that the MAPK activation (both peaks) triggered by UV-oxLDL does not require RNA and protein synthesis (e.g. synthesis of growth factors).

Then, to investigate the potential involvement of growth factors in the mitogenic effect of UV-oxLDL, two additional sets of experiments were performed using antibodies against growth factors and transfer of preconditioned medium (Tables 2 and 3). As shown in Table II, under the experimental conditions used here, PDGF exhibited a mitogenic effect, whereas bFGF and EGF were not significantly mitogenic to AG-08133A SMC. Moreover, neutralizing antibodies (anti-PDGF, anti-bFGF, and anti-EGF antibodies able to block the mitogenic effect of human and bovine growth factors) did not inhibit the mitogenic effect of UV-oxLDL (Table II).

                              
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Table II
Effect of neutralizing antibodies against PDGF, EGF, and bFGF on AG-08133A SMC proliferation induced either by exogenous growth factors or by UV-oxidized LDL
[3H]Thymidine incorporation was evaluated under standard conditions and expressed as percent of the control (i.e. cells grown in the absence of any exogenous growth factor or UV-oxLDL). Mean ± S.E.M. of four experiments.

In a separate set of experiments, preconditioned medium (from SMC treated with UV-oxLDL) was transferred to untreated (reporter) SMC to test its potential mitogenic effect. The preconditioned medium was prepared as follows. AG-08133A SMC were "pulsed" for variable periods of time with a mitogenic concentration of UV-oxLDL. Then, this pulse medium was discarded; after washing, the SMC were "chased" for 2 or 4 h in UV-oxLDL-free medium that was used as preconditioned medium. These preconditioned media were immediately transferred to reporter AG-08133A SMC. Preconditioned media (UV-oxLDL-free) exhibited no or only poorly mitogenic activity (Table III).

                              
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Table III
Effect of preconditioned ("chase") culture media (from AG-08133A SMC preincubated with UV-oxLDL) on MAPK activity and [3H]thymidine incorporation of reporter AG-08133A SMC
Preconditioned media were prepared as follows. SMC were preincubated (or "pulsed") for 1 or 16 h in RPMI containing 1% FCS and 100 µg of apoB/ml of UV-oxLDL; then, this medium (containing UV-oxLDL) was discarded, and SMC were incubated ("chased") for an additional 2 or 4 h in RPMI containing 1% FCS (preconditioned culture medium). The preconditioned media ("chase" media) were then transferred to reporter AG-08133A SMC. After addition of the preconditioned medium, the MAPK activities and [3H]thymidine incorporation were determined on the reporter SMC, at 1 and 3 h for MAPK (time of the MAPK peaks evoked by UV-oxLDL) and 16 h for [3H]thymidine incorporation. Mean ± S.E.M. of three to five experiments.

Together, these data suggest that, in our model system, the mitogenic effect of UV-oxLDL is probably not mediated by secreted (autocrine) mediators, such as growth factors.

Potential Role of Ceramide in MAPK Activation Evoked by UV-oxLDL-- Proliferation of vascular SMC induced by mitogenic doses of UV-oxLDL has been shown to be associated with the activation of the SM-ceramide pathway and to be mimicked by short chain permeant ceramides (11). Here, we show that SM hydrolysis was associated with the activation of a neutral SMase, whereas SMase activities at acidic and alkaline pH remained unchanged (Fig. 3A). The neutral SMase activated by UV-oxLDL was not affected by the presence of EDTA in the reaction buffer (data not shown), thus suggesting that this neutral SMase is magnesium-independent.


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Fig. 3.   Relative time course of SMase activation, SM hydrolysis, ceramide generation, and MAPK activation in AG-08133A SMC treated by UV-oxLDL (100 µg of apoB/ml) and inhibition by 10 µM serpins TPCK and DCIC (empty squares and triangles, respectively).  A, time course of SMase activation elicited by UV-oxLDL. SMC were incubated for 48 h in RPMI medium containing 1% FCS. Then, the medium was replaced by fresh medium containing UV-oxLDL (100 µg of apoB/ml). At the indicated times, SMase activities were determined under the conditions described under "Experimental Procedures." Neutral SMase activity was determined at pH 7.4 in the presence of 10 mM EDTA (bullet ), acid SMase activity at pH 5.0 (black-square), and alkaline SMase activity at pH 8.5 (black-triangle). SMase activities were expressed as percent of the value at time 0 (i.e. 74 ± 6, 51 ± 4, and 2290 ± 130 pmol/h·mg cell protein for the neutral, alkaline, and acid SMases, respectively). B, inhibition by serpins of the neutral SMase activated by UV-oxLDL. SMC were starved for 48 h in RPMI medium containing 1% FCS. The medium was discarded, and cells were preincubated in fresh medium without (bullet ) or with serpins for 2 h (10 µM TPCK (square ) or DCIC (triangle )), just before addition (time 0) of 100 µg of apoB/ml of UV-oxLDL. At the indicated times, cells were harvested and immediately used for determining neutral SMase activity under the conditions used in A. C and D, SM hydrolysis and ceramide generation induced by UV-oxLDL is inhibited by serpins. SMC were preincubated for 48 h in RPMI medium containing 1% FCS and [methyl-3H]choline (0.5 µCi/ml) (in C) or [3H]palmitic acid (0.5 µCi/ml) (in D) and then treated under the same conditions as in B. At the indicated times, cells were harvested and lipids extracted for determining radiolabeled SM and ceramide levels as described under "Experimental Procedures." Results are expressed as percent of values at time 0. E, MBP kinase activation induced by UV-oxLDL is inhibited by serpins. SMC were treated under the conditions of B; at the indicated time, cells were harvested for determining MBP kinase activity. F, cell viability of SMC incubated for 5 h (black bars) and 24 h (gray bars) under the conditions of B, i.e. in basic culture medium (controls, Co), in media containing UV-oxLDL (oxL) or UV-oxLDL plus TPCK (oxL + T) or UV-oxLDL plus DCIC (oxL + D). Cell viability was evaluated by trypan blue exclusion and expressed as unstained cells percent. Mean ± S.E. of three to five experiments.

In an attempt to understand whether the activation of the SM-ceramide and MAPK pathways triggered by UV-oxLDL were independent or causally related, two sets of experiments were designed using SM hydrolysis inhibitors and exogenous ceramide.

Serine protease inhibitors (serpins) have recently been shown to be able to block the activation of the SM-ceramide pathway involved in daunorubicin-induced apoptosis (47). In our experimental model system, effective concentrations of the two serpins used here, DCIC and TPCK, inhibited concomitantly SMase stimulation (Fig. 3B), SM hydrolysis (Fig. 3C), ceramide production (Fig. 3D), MAPK activation (Fig. 3E), and [3H]thymidine incorporation (Table IV) induced by mitogenic concentrations of UV-oxLDL (100 µg of apoB/ml). Finally, we examined whether the inhibitory effect of serpins on [3H]thymidine incorporation may result from a broad toxic effect. Over the time of experiment (5 h), we did not detect any significant toxicity of the two serpins (at the used concentrations, 10 µM) (Fig. 3F). In longer time-course experiments (24 or 48 h), DCIC was not toxic to SMC, and TPCK was only slightly toxic, as evaluated by trypan blue staining. Therefore, the inhibitory effect of TPCK or DCIC on [3H]thymidine incorporation in SMC treated by UV-oxLDL (Table IV) does not seem to result from a toxic effect but rather from an inhibition of [3H]thymidine incorporation. To investigate whether this inhibitory effect was a general effect of protease inhibitors or was relatively specific to TPCK or DCIC, we examined the effect of other protease inhibitors (which inhibit necrosis or apoptosis induced by UV-oxLDL) (48). As reported in Table IV, leupeptin, antipain, and pepstatin A were ineffective in contrast to TPCK or DCIC.

                              
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Table IV
Effect of protease inhibitors on SM hydrolysis and [3H]thymidine incorporation induced by mitogenic concentrations of UV-oxLDL
Mean ± S.E.M. of three experiments.

As C2-ceramide and ceramide generated at the plasma membrane by bacterial SMase treatment are mitogenic to SMC (11), we investigated the potential role of ceramides in the activation of MAPK. SMase treatment, used under non-lytic conditions leading to SM hydrolysis and ceramide generation in the plasma membrane (11), elicited a biphasic activation of MBP kinase and enhanced [3H]thymidine incorporation (Fig. 4). In contrast, treatment of cells by bacterial phospholipase C (PLC, used under non-lytic conditions leading to about 40% hydrolysis of cellular phosphatidylcholine without significant hydrolysis of SM) (11) induced no significant activation of MBP kinase nor [3H]thymidine incorporation (Fig. 4).


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Fig. 4.   Activation of MBP kinase and [3H]thymidine incorporation induced by bacterial SMase or PLC from B. cereus. A, time course of MBP kinase activation in response to treatment by bacterial SMase (black-square) or PLC (black-triangle). SMC, starved in RPMI 1640 containing 1% FCS for 48 h, were then treated by SMase (100 milliunits/ml for 1 h) or PLC (200 milliunits/ml for 1 h). At the indicated times, MBP kinase activity was determined as detailed under "Experimental Procedures" after immunoprecipitation of MAPK (by using anti-ERK1/ERK2 antibody) and expressed as nmol/min/mg of protein of the cell homogenate. Mean ± S.E. of three experiments. B, [3H]thymidine incorporation was evaluated at time 24 (black bars) and 48 h (hatched bars) under conditions described in "Experimental Procedures" and expressed as percent of the control. Mean ± S.E. of four experiments.

Similarly, the synthetic short chain permeant C2-ceramide induced a biphasic activation of the MBP kinase (Fig. 5A) and enhanced [3H]thymidine incorporation (Fig. 5B). In contrast, C2-dihydroceramide (DHC), an inactive analog of C2-ceramide, used under conditions similar to C2-ceramide, did not activate MBP kinase nor increase [3H]thymidine incorporation (Fig. 5, A and C). The data of Figs. 4 and 5 suggest that MAPK activation and [3H]thymidine incorporation induced by SMase treatment or by C2-ceramide did not result from a nonspecific effect, as bacterial PLC and DHC were inactive.


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Fig. 5.   Activation of MBP kinase and [3H]thymidine incorporation induced by the exogenous cell permeant C2-ceramide and effect of inhibitors. A, time course of MBP kinase activity in response to 2.5 µM C2-ceramide (C2-cer) or dihydroceramide (C2-DHC). B, effect of inhibitors on C2-ceramide-induced MBP kinase activation. SMC, starved for 48 h in RPMI 1640 containing 1% FCS, were treated with 2.5 µM C2-ceramide (C2) or DHC and inhibitors (10 µM) when indicated. Then, MBP kinase activity was evaluated at time 30 min (gray bars) or 3 h (striped bars) under conditions of A. Mean ± S.E. of three experiments. C, [3H]thymidine incorporation induced by C2-ceramide or C2-dihydroceramide and effect of inhibitors. SMC were treated by 2.5 µM C2-ceramide (C2) or DHC and 10 µM inhibitors when indicated (P, PD-098059; T, TPCK; D, DCIC). [3H]Thymidine incorporation was evaluated after 24 (black bars) and 48 h (hatched bars) of incubation, under conditions described under "Experimental Procedures." Mean ± S.E. of four experiments.

Effective concentration of the MAPK kinase inhibitor PD-098059 abrogated both the MAPK activation and [3H]thymidine incorporation elicited by C2-ceramide (Fig. 5, B and C), thus suggesting that [3H]thymidine incorporation evoked by C2-ceramide is dependent on MAPK activation. In contrast, TPCK and DCIC did not inhibit significantly the MAPK activation and the mitogenic effect elicited by the cell-permeant short chain ceramide (Fig. 5, B and C). Together, these data strongly suggest that, in this experimental model system, serpins inhibit the UV-oxLDL-induced ceramide production (probably by acting upstream from SM hydrolysis) and subsequently [3H]thymidine incorporation.

    DISCUSSION
Top
Abstract
Introduction
Procedures
Results
Discussion
References

The present study shows that, in cultured vascular AG-08133A SMC, (i) mitogenic concentrations of UV-oxLDL elicit the activation of the SM-ceramide pathway and the stimulation and nuclear translocation of MAPK and (ii) ceramides (natural ceramide generated in the plasma membrane by SMase treatment or short chain permeant C2-ceramide) are effective mitogenic mediators, which are also able to induce activation and nuclear translocation of MAPK and subsequent stimulation of [3H]thymidine incorporation.

Oxidized LDL have been shown to induce a significant increase of [3H]thymidine incorporation and proliferation of cultured aortic SMC (9-11). This mitogenic effect is stronger than that of native LDL (10, 11), which were only poorly mitogenic to SMC, despite their ability to induce some intracellular signaling (49).

Moderate concentrations of UV-oxLDL (100 µg of apoB/ml) induced a significant mitogenic response in vascular SMC, in a medium supplemented with either human lipoprotein-depleted serum (10) or 1% FCS (11). In G0-arrested cells, initiation of DNA synthesis is a complex process that requires potent growth factors enabling cells to pass the G1 restriction point controlling S phase entry (50). We report here that, similarly to growth factors, the proliferative effect of UV-oxLDL on SMC was associated with a biphasic, sustained stimulation of MBP kinase activity, tyrosine phosphorylation. and nuclear translocation of p44/p42 MAPKs. In contrast, native LDL induced only a transient activation of MAPK. The role of MAPK activation in the proliferation of SMC induced by UV-oxLDL was supported by the inhibitory effect of PD-098059, a MAPK kinase inhibitor, which blocked both the MAPK activation (45) and the SMC proliferation.

An early and transient activation of MAPK has been reported to be induced by native LDL (44, 51, 52) or oxLDL (44, 52-54), but, in these studies, no information was provided on the late events (over 5 h) and nuclear translocation of MAPK, which are thought to play a key role in the full mitogenic response (55). When monitoring the MAPK activation during a longer period of time, we observed an obvious difference between MAPK activation triggered by native LDL and UV-oxLDL, as only UV-oxLDL induced the biphasic and sustained activation of MAPK. This response is quite similar to that observed with classical mitogens that induce a full mitogenic response (30, 31, 55).

We therefore considered the possibility that oxidized LDL may promote indirectly cell growth via an auto/paracrine mechanism resulting from enhanced expression of growth factors. Several data obtained suggest that a role of autocrine growth factors is unlikely in our model system (cultured vascular AG-08133A SMC used under the described experimental conditions). (i) The interval of time between cell contact with and MAPK activation by UV-oxLDL (the first peak occurred after a 1-h pulse with UV-oxLDL) is relatively short for an autocrine signaling involving stimulation of growth factor synthesis by UV-oxLDL. For instance, as oxLDL-induced PDGF-A mRNA peaked after 2 h of incubation (49) and protein synthesis and secretion of PDGF need some additional time, PDGF secretion cannot explain the MAPK activation occurring at 1 h. (ii) Similarly, MAPK activation triggered by exogenous SMase (which mimics the mitogenic effect of UV-oxLDL) occurs very rapidly (first peak at 5 min), thereby excluding a role of growth factors (gene induction, protein synthesis, and secretion of growth factors being very unlikely in this very short time). (iii) Inhibition of mRNA or protein synthesis by effective doses of actinomycin D or cycloheximide did not block the MAPK activation induced by UV-oxLDL. (iv) MAPK activation by ceramide (ceramide generated by SMase and permeant C2-ceramide) was not abrogated by actinomycin D or cycloheximide (data not shown). (v) Blocking antibodies against PDGF, bFGF, and EGF (used under conditions inhibiting the response induced by the related growth factor) did not affect the MAPK activation nor the mitogenic response triggered by UV-oxLDL. Moreover, in agreement with Stiko-Rahm et al. (49), when the preconditioned medium (obtained by preincubating SMC with oxLDL) was transferred on reporter SMC, no significant mitogenic effect was observed. Taken together, these data strongly suggest that an autocrine secretion of growth factors triggered by oxLDL plays only a minor role in our model system. Therefore, from our recently reported data (11), we hypothesized that UV-oxLDL may act directly as a mitogen to SMC by triggering the SM-ceramide pathway and subsequently the MAPK cascade. Of course, these data do not exclude the possibility that, in atherosclerotic lesions, growth factors may play a prominent role in the genesis of lesions (see review in Ref. 6).

The identification of SMase(s) involved in ceramide generation has proven to be equivocal. At least three forms of SMase are candidates for SM hydrolysis. Acid SMase has been associated with signaling triggered by TNFalpha (39), Fas (19), and CD28 (18). Activation of a membrane-bound neutral SMase has also been described with TNFalpha (39), anti-Fas antibody (20), and daunorubicin (21). Finally, a cytosolic magnesium-independent neutral SMase has been implicated in vitamin D3-induced differentiation (56). In our study, UV-oxLDL induced only activation of a neutral SMase (peaking at 1 h), which may be similar to the enzyme described by Okazaki et al. (56). The activation of the neutral SMase was inhibited by TPCK and DCIC concomitantly with SM hydrolysis and ceramide generation, thus suggesting that the neutral SMase is involved in SM hydrolysis and mitogenic signaling triggered by UV-oxLDL. These data are consistent with the role of this SMase in the TNFalpha -induced mitogenic signaling in fibroblasts (38). The molecular mechanism of the activation of this neutral SMase by oxLDL remains unknown, but its inhibition by serpins (Ref. 47 and present paper) or by caspase inhibitors (57, 58) supports the hypothesis for a role of protease(s) in SMase activation.

Furthermore, the two serpins TPCK and DCIC inhibited concomitantly ceramide generation (subsequent to SM hydrolysis), MAPK activation, and [3H]thymidine incorporation triggered by UV-oxLDL but did not inhibit the MAPK activation and mitogenic effect induced by short chain ceramide. Taken together, these data suggest that serpins act upstream from the SMase, and do not interfere, in our model system, between ceramide and downstream signaling, i.e. MAPK activation and DNA synthesis.

Another major question is to know whether the activation of the SM-ceramide pathway is involved in the mitogenic effect or is only a parallel consequence of the response of cells to UV-oxLDL. The former hypothesis is supported by the fact that both MAPK activation and mitogenic effect of UV-oxLDL were mimicked by exogenous short chain permeant ceramide and by ceramide generated at the plasma membrane by exogenous SMase. A nonspecific effect of these mediators (for instance membrane damages triggering the activation of the MAPK pathway) is unlikely because (i) phospholipid hydrolysis by exogenous phospholipase C did not trigger MAPK activation or DNA synthesis, although it induced probably plasma membrane structural changes similar to those elicited by SMase, and (ii) C2-dihydroceramide was ineffective, in contrast to C2-ceramide.

Together, the above reported data are consistent with the hypothesis that UV-oxLDL may induce the sequential activation of the SM-ceramide pathway, MAPK cascade, and downstream mitogenic signaling. This is consistent with Raf1 phosphorylation (59) and MAPK activation induced by endogenous or cell-permeant ceramides in HL60 leukemic cells (60, 61), fibroblasts (62, 63), and endothelial cells (64). Although MAPK activation by ceramide has been demonstrated in cellular systems undergoing apoptotic or inflammatory responses, our results strongly implicate activation of MAPK by ceramide in a proliferative signaling pathway consistent with the well documented mitogenic role of MAPK (30, 31, 55).

In various experimental models, other sphingolipid mediators such as lactosylceramide, sphingosine 1-phosphate, or sphingosylphosphocholine have been shown to stimulate the p42/p44 MAPK or exert a proliferative effect (54, 65-67). The possibility that, in our model system, ceramide may be degraded and converted into sphingosine 1-phosphate or sphingosylphosphocholine, or utilized as a precursor for lactosylceramide biosynthesis, cannot be ruled out. To date, the respective role of the ceramide pathway and other pathways involving other sphingolipid mediators in the oxLDL-induced mitogenic effect remains to be elucidated.

In conclusion, the present paper reports several novel results concerning the mitogenic intracellular signaling triggered by oxLDL in vascular SMC. (i) The mitogenic effect of UV-oxLDL is mediated through serpin-sensitive serine proteases, which activate in turn the SM-ceramide pathway. (ii) The mitogenic effect resulting from the activation of the SM-ceramide pathway is mediated through a biphasic and sustained activation and nuclear translocation of MAPK. Finally, our data suggest that the activation of SM-ceramide pathway induces in turn a sustained activation of the MAPK pathway, associated with nuclear translocation of MAPK, which is a critical event during G1 progression (55) and seems to be sufficient for inducing cell proliferation (68). As oxLDL are present in atherosclerotic lesions, but not in normal vascular wall (7), this mitogenic stimulus is locally persistent and specific to atherosclerotic areas. It is therefore suggested that, besides the other cytokines and growth factors potentially involved in atherogenesis (6), oxLDL may play a critical role in the proliferation of SMC occurring in atherosclerotic plaque.

    ACKNOWLEDGEMENT

We thank C. Mora for technical assistance.

    FOOTNOTES

* This work was supported in part by grants from INSERM, Université Paul Sabatier, Conseil Régional Midi-Pyrénées, Fondation pour la Recherche Médicale (to R. S.), and Fédération Nationale des Centres de Lutte contre le Cancer (to T. L.).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.

§ These authors contributed equally to this work.

Fellowship recipients from the Ministère de l'Education Nationale.

parallel Fellowship recipient from Vaincre les Maladies Lysosomales.

** Fellowship recipient from Association Française contre les Myopathies.

§§ To whom correspondence should be addressed. Tel.: 33-561-32-31-48; Fax: 33-561-32-20-84; E-mail: salvayre{at}rangueil.inserm.fr.

1 The abbreviations used are: SMC, smooth muscle cells; LDL, low density lipoproteins; oxLDL, oxidized LDL; MAPK, mitogen-activated protein kinase; C2-Cer or C2-ceramide, N-acetyl-D-sphingosine; SM, sphingomyelin; SMase, sphingomyelinase; PLC, phospholipase C; MBP, myelin basic protein; TPCK, N-tosyl-L-phenylalanyl chloromethyl ketone; DCIC, dichloroisocoumarin; EGF, epidermal growth factor; PDGF, platelet-derived growth factor; bFGF, basic fibroblast growth factor; FCS, fetal calf serum; PBS, phosphate-buffered saline; PMSF, phenylmethylsulfonyl fluoride; DHC, C2-dihydroceramide; TNFalpha , tumor necrosis factor-alpha ; ERK, extracellular regulated kinase.

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Top
Abstract
Introduction
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Results
Discussion
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