|
|
|
|
|
|
|
||
Article |
Remodeling of cellular cytoskeleton by the acid sphingomyelinase/ceramide pathway
Correspondence to Yusuf A. Hannun: hannun{at}musc.edu
The chemotherapeutic agent cisplatin is widely used in treatment of solid tumors. In breast cancer cells, cisplatin produces early and marked changes in cell morphology and the actin cytoskeleton. These changes manifest as loss of lamellipodia/filopodia and appearance of membrane ruffles. Furthermore, cisplatin induces dephosphorylation of the actin-binding protein ezrin, and its relocation from membrane protrusions to the cytosol. Because cisplatin activates acid sphingomyelinase (ASMase), we investigate here the role of the ASMase/ceramide (Cer) pathway in mediating these morphological changes. We find that cisplatin induces a transient elevation in ASMase activity and its redistribution to the plasma membrane. This translocation is blocked upon overexpression of a dominant-negative (DN) ASMaseS508A mutant and by a DN PKC
. Importantly; knockdown of ASMase protects MCF-7 cells from cisplatin-induced cytoskeletal changes including ezrin dephosphorylation. Reciprocally, exogenous delivery of D-e-C16-Cer, but not dihydro-C16-Cer, recapitulates the morphotropic effects of cisplatin. Collectively, these results highlight a novel tumor suppressor property for Cer and a function for ASMase in cisplatin-induced cytoskeletal remodeling.
 |
Introduction |
|---|
 TopAbstract Introduction ResultsDiscussionMaterials and methodsReferences |
|---|
The actin cytoskeleton and its associated proteins are essential players in cell motility, adhesion, and morphogenesis. Ezrin, a member of the ERM family, regulates cytoskeletal dynamics by cross-linking actin filaments to the plasma membrane (Bretscher et al., 2002; Fievet et al., 2007). Two cellular forms of ezrin have been studied: an inactive cytoplasmic form and an active membrane-bound form. In its inactive conformation, the N-terminal membrane association domain of ezrin exerts intramolecular masking of the actin-binding domain located at the C terminus. Sequential binding of the phosphoinositide PIP2 at the N terminus followed by phosphorylation of the C-terminal threonine 567 residue results in unmasking of the functional protein binding sites, thus allowing ezrin to associate simultaneously with the cytoplasmic tail of various transmembrane proteins and with F-actin (Fievet et al., 2004). In its active form, ezrin promotes formation of specialized cellular protrusions such as lamellipodia, filopodia, and microvilli, essential structures in motility and contact with other cell types.
Effectors of ceramide signaling have been implicated in regulating cellular motility. In particular several studies have correlated the ceramide-activated serine/threonine phosphatase PP2A with decreased tumor metastasis (Metz et al., 1996; Meisinger et al., 1997). Xu and Deng (2006) recently reported that loss of PP2A increases migration and invasion of lung cancer cells. Treatment with C2-ceramide, a potent PP2A agonist, suppressed motility of cancer cells (Xu and Deng, 2006). However, the underlying mechanisms by which PP2A affects tumor cell motility remain unknown.
To understand the molecular mechanisms by which sphingolipids influence cellular architecture, we investigated the effects of stress-induced endogenous ceramide generation in MCF-7 breast cancer cells, using cisplatin, a chemotherapeutic agent of major clinical utility for treatment of breast cancer.
We demonstrate here that ceramide production plays an important role in stress-induced cytoskeletal remodeling. Cisplatin induced marked changes in the actin cytoskeleton, including dephosphorylation and cytosolic translocation of ezrin. Mechanistically, activation of acid sphingomyelinase (ASMase) is shown to be required upstream of the observed morphological changes. Further investigation revealed a novel association between ceramide-activated PP2A and ezrin at the plasma membrane. These findings demonstrate that the ASMase/ceramide pathway is instrumental for cytoskeletal remodeling induced by chemotherapeutic interventions.
|
Results |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and methodsReferences |
|---|
|
|
Cisplatin activates the ASMase/ceramide pathway
The effects of cisplatin on dephosphorylation of ezrin raised the possibility of activation of a serine/threonine phosphatase. Importantly, previous studies have shown that the bioactive lipid ceramide activates phosphatases in vitro and in cells (Pettus et al., 2002). Moreover, the ASMase/ceramide pathway has been previously shown to be activated by cisplatin (Levade and Jaffrezou, 1999; Lacour et al., 2004). Therefore, it became important to evaluate whether the observed changes with cisplatin are due to modulation of sphingolipid metabolism. To that end, MCF-7 cells were treated with cisplatin (5 µg/ml) over a time course of 3 h, and sphingolipids were extracted by the Bligh Dyer technique. Mass spectrometric measurements revealed a transient elevation in total ceramide (twofold) within 30 min of cisplatin treatment (Fig. 3 A).
Further analysis indicated that this change was mainly accounted for by an increase in ceramide species carrying C16 and C24:1 acyl chains (Fig. 3 C). Importantly, the observed changes in ceramide levels were paralleled by a transient drop in sphingomyelin (SM) levels (Fig. 3 B). In particular, a major change in C16 SM and a minor one in C24:1 SM were detected by mass spectrometry after 15 min of cisplatin treatment (Fig. 3 D). Together, this sphingolipidomic profile suggests the operation of a sphingomyelinase.
|
|
ASMase is upstream of ezrin dephosphorylation and the cytoskeletal changes
Given the above results, it became important to investigate whether changes in sphingolipid metabolites mediate the action of cisplatin. Therefore, knockdown of ASMase was attempted using RNAi technology. Two different 21-bp oligonucleotides targeting ASMase or a control (scrambled) sequence were transfected into MCF-7 cells. Western blotting confirmed loss of the ASMase protein (>70%) after 48 h of RNAi transfection (Fig. 5 A). Importantly, knockdown of ASMase blocked cisplatin-induced ezrin dephosphorylation as determined by Western blotting (Fig. 5 B).
This result prompted us to define the role of ASMase in cisplatin-induced cytoskeletal changes. To this end, cells were transfected with either ASMase RNAi or SCR oligonucleotides for 48 h. Confocal microscopy imaging revealed that cisplatin treatment caused an overall rounding, loss of cellular filopodia, and relocation of ezrin to a more cytosolic distribution in the control group (SCR). It is worth noting that a normal nuclear morphology was maintained (red channel), suggesting that the observed changes are not secondary to cell death. Importantly, cells transfected with ASMase RNAi were remarkably protected from the morphological effects of cisplatin. This was indicated by retention of not only cellular filopodia but also peripheral ezrin localization after cisplatin treatment (Fig. 5 C). Therefore, these findings suggest a critical role for ASMase in mediating the cytoskeletal effects of cisplatin.
|
|
PP2A mediates ezrin dephosphorylation
Ceramide-activated protein phosphatases (CAPPs) are well established effectors of ceramide generating pathways of which PP2A and PP1 remain the best studied thus far (Ruvolo, 2003). Therefore, it became important to determine whether the observed dephosphorylation of ezrin is mediated by CAPPs. In previous studies, it was demonstrated that okadaic acid potently inhibits PP2A when used at low doses (Chalfant et al., 1999, 2001). Cells were pretreated with either okadaic acid (10 nM) or vehicle (DMSO) 1 h before cisplatin addition. Western blot analysis revealed that inhibition of PP2A with okadaic acid restored levels of p-ezrin (Fig. 7 A). We also entertained the potential involvement of another well-established ceramide activated phosphatase, PP1. However, treatment with tautomycin (10 nM), a specific PP1 inhibitor, had little effect on cisplatin-induced ezrin dephosphorylation (Fig. 7 B).
These results were further corroborated using RNAi technology. For these experiments, MCF-7 cells were transfected with 20 nM of either control (SCR) or PP2A-specific 21-bp oligonucleotides. After 48 h, marked knockdown (>70%) of PP2A protein was observed by Western blotting (Fig. 7 C). Importantly, loss of PP2A conferred protection from cisplatin-induced ezrin dephosphorylation (Fig. 7 C). These findings provide strong pharmacologic and genetic evidence for PP2A in ezrin dephosphorylation.
|
PKC mediates activation of ASMase by cisplatin
Recently, we defined a mechanism for ASMase activation in which PKC serves as a key upstream kinase (Zeidan and Hannun, 2007). Therefore, we investigated whether cisplatin treatment modulated PKC activity in MCF-7 cells. In vitro kinase assays revealed a significant elevation (1.5-fold) in PKC activity by 30 min and further elevation (3-fold) after 1 h of cisplatin treatment (Fig. 8 A). Because this time frame of PKC induction is consistent with the kinetics of ASMase activation by cisplatin, the role of PKC in this process was evaluated. Therefore, cells were infected with either control adenoviruses (LacZ) or viruses encoding a dominant-negative construct of PKC (DN-PKC) before stimulation with cisplatin.
In comparison with the control group, cells infected with DN-PKC showed a significant reduction in ASMase activity after cisplatin treatment (Fig. 8 B). Additionally, the effect of DN-PKC on cisplatin-induced ASMase relocation was evaluated. The results revealed a 40% drop (65% inhibition of the response) in cells showing plasma membrane translocation of ASMase after cisplatin treatment (Fig. 8 C).
|
.
ASMase mediates the effect of cisplatin on cell migration
Recent studies have indicated a major role for ezrin in regulating cellular motility (Fievet et al., 2007; Prag et al., 2007). In particular, the active phosphorylated form of ezrin is tumor promoting as it enhances cellular migration and invasion. Therefore, we hypothesized that inactivation of ezrin by cisplatin treatment influences cellular motility. This hypothesis was tested using a wound-healing assay applied to confluent monolayers of MCF-7 cells stably overexpressing WT ASMase or ASMaseS508A. As shown in Fig. 9 A, under basal conditions both ASMase and ASMaseS508A stables were able to reduce the wound to 27% of its original size after 48 h. Importantly, the wound-healing ability of cells incubated with cisplatin (5 µg/ml) was markedly reduced to only 70% of original wound size, indicating reduced migration in the presence of cisplatin.
On the contrary, cells overexpressing ASMaseS508A were significantly refractory to the effects of cisplatin, as they were still able to reduce wound size to 40%. Importantly, ASMaseS508A cells were also refractory to ezrin dephosphorylation and cytosolic translocation after cisplatin treatment as compared with WT-ASMase cells (Fig. S2, A and B; available at http://www.jcb.org/cgi/content/full/jcb.200705060/DC1). Together, these findings strongly suggest that suppression of cellular motility by cisplatin requires activation of ASMase.
|
|
Discussion |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and methodsReferences |
|---|
upstream of ASMase and for PP2A downstream of ceramide in the dephosphorylation of ezrin. Functionally, dephosphorylation/inactivation of ezrin correlated with reduced mobility of MCF-7 cells after cisplatin treatment in an ASMase-dependent manner. Collectively, these results identify a novel pathway involving ASMase/ceramide in mediating stress responses on the actin cytoskeleton. A major conclusion from this study emanates from defining a novel molecular/biochemical mechanism for ezrin inactivation. Previous studies demonstrated that binding of the phosphoinositide PIP2 at the N terminus of ezrin facilitates its conformational change (Fievet et al., 2004). However, reciprocal regulation (inactivation) of ezrin by other bioactive lipids and by other pathways remains largely unknown. The data presented here suggest that the ASMase/ceramide pathway mediates stress-induced ezrin dephosphorylation and consequent retraction of filopodia (Fig. 10, model). This model is supported by several lines of evidence. First, cisplatin activated ASMase and induced ceramide in a time course consistent with a role upstream of ezrin dephosphorylation. Second, genetic knockdown of ASMase blocked ezrin dephosphorylation and restored cellular morphology after cisplatin treatment. Third, cells overexpressing DN ASMaseS508A maintained levels of p-ezrin after cisplatin treatment and, more importantly, preserved their migratory response in a wound-healing model. Finally, addition of exogenous ceramide mimicked the morphotropic effects of cisplatin including dephosphorylation of ezrin.
|
The results from this study also significantly extend the spectrum of stress responses mediated by ceramide. Modulation of sphingolipid metabolism is emerging as a shared cellular stress response to chemotherapy (Bezombes et al., 2003; Marchesini and Hannun, 2004). In particular, the ASMase/ceramide pathway has been suggested as a target for different classes of cytotoxic drugs including: DNA damaging agents (doxorubicin [Herr et al., 1997]), histone deacetylase inhibitors (Rahmani et al., 2005), fenretinide (Lovat et al., 2004), and microtubule-targeting agents (paclitaxel [Prinetti et al., 2006]). Activation of ASMase by these agents has been associated with apoptotic cell death. Although the actions of chemotherapies are not limited to cell killing, the role of ASMase in responses other than cytotoxicity have not been well studied. For the first time, the results presented in this study demonstrate that ASMase hinders the mobility of mammalian cells through remodeling of the cellular cytoskeleton.
The present study established that ceramide signaling mediates the cytoskeletal rearrangement produced by cisplatin. Recently, identification of the morphotropic properties of ceramide and other bioactive sphingolipids has emerged as an important goal. Sphingosine-1-phosphate (S1P), a catabolite of ceramide, elicits profound cytoskeletal effects mainly through regulating Rho GTPases (Toman et al., 2004; Donati and Bruni, 2006). Although an increase in ceramide and a drop in S1P may be detrimental for cell survival (Maceyka et al., 2002), the current study suggests that the bioactive lipid ceramide also governs cellular morphology and its associated biological processes. For the first time, we show that ceramide modulates the actin cytoskeleton by inducing dephosphorylation of ezrin. These changes seem to be specific to ceramide, as the inactive dihydroceramide analogue failed to dephosphorylate ezrin. Using the same cell line used in this study, Panigone et al. (2001) observed that up-regulation of prosaposin, an activator of ASMase, or treatment with C2-ceramide, causes defective cell spreading and impaired adhesion. Such cytoskeletal responses elicited by ceramide do not seem to be specific for MCF-7 cells, as similar observations have been made by other investigators in different cell lines. In a recent study, Hu et al. (2005) demonstrated that exogenous C6-ceramide induced loss of filopodia in HeLa cells. The divergence of the morphological effects of ceramide from apoptosis was demonstrated by Spinedi and coworkers, as caspase inhibitors blocked only cell death but not detachment (Di Bartolomeo and Spinedi, 2002). With this in mind, one can propose that ceramide derives its tumor suppressor properties from being not only a pro-apoptotic lipid, but also a morphotropic one.
The results from this study also significantly extend our understanding of signaling mechanisms both upstream and downstream of ASMase. Upstream, the results implicate PKC in this pathway. Although activation of ASMase was reported to be a critical step for cisplatin-induced ceramide generation (Lacour et al., 2004), the molecular mechanism underlying this process is not known. A critical role for PKC in mediating activation of ASMase by cisplatin is supported by several lines of evidence. In vitro enzymatic assays revealed similar kinetics for ASMase and PKC activation after cisplatin treatment. Additionally, infection with DN-PKC adenovirus impaired not only activation but also membrane translocation of ASMase in response to cisplatin. These results are in concert with our recently reported mechanism of ASMase regulation (Zeidan and Hannun, 2007) in which activation of ASMase proceeds through PKC-mediated phosphorylation of the enzyme at S508. The validity of this model is further corroborated by the finding that the ASMaseS508A mutant failed to translocate to the plasma membrane after cisplatin treatment.
As to downstream mechanisms, the identification of ezrin as a target for PP2A-mediated dephosphorylation extends the current understanding of PP2A as a regulator of cellular motility. Previous work from our laboratory and others established PP2A as a lipid-binding phosphatase that is activated upon ceramide binding to its catalytic domain (Chalfant et al., 1999, 2004). Although the catalytic activity of PP2A has been tightly associated with reduced cellular motility in various tumors, there is little molecular understanding of this process. The present study proposes regulation of ezrin as a key mechanism by which PP2A limits cellular motility. First, targeting PP2A using pharmacologic (okadaic acid) and genetic approaches (RNAi) blocked ezrin dephosphorylation. Second, FRET experiments uncovered an association of PP2A and ezrin at the cell membrane in response to cisplatin. Furthermore, dephosphorylation of ezrin at Thr 526 seemed to be specifically carried by PP2A but not PP1, another ceramide-activated phosphatase, as inhibition of PP1 with tautomycin did not rescue levels of p-ezrin. It is worth noting that dephosphorylation of ERM proteins has been previously reported in response to chemokines such as SDF (Brown et al., 2003), FMLP, and GM-CSF (Yoshinaga-Ohara et al., 2002), but the identities of the phosphatases involved were not established.
Based on the current findings, ASMase emerges as a novel extranuclear target for cisplatin action. Although classically regarded as a nuclear DNA damaging agent, recent studies support a more promiscuous mode of cisplatin action. Safaei et al. (2005) demonstrated that fluorescently labeled cisplatin concentrates within lysosomes. Additional evidence suggests that cisplatin targets lysosomal proteases such as cathepsin D (Emert-Sedlak et al., 2005). Interestingly, cathepsin D has been previously shown as a downstream protease of ASMase activation and a key ceramide-binding protein (Heinrich et al., 1999, 2000, 2004). Although we did not directly address whether activation of ASMase by cisplatin is mediated by a nuclear signal, a recent study by Charruyer et al. (2005) demonstrating activation of ASMase in platelets after UV radiation supports a model of ASMase that is independent of nuclear signaling. Of note, other reports have shown intact cytotoxic effects of cisplatin in enucleated cells (cytoplasts) (Mandic et al., 2003).
In conclusion, the results in this study demonstrate that the ASMase/ceramide pathway conveys stress signals to the actin cytoskeleton machinery. The study unveils a novel sphingolipid-mediated mechanism of ezrin regulation. Based on these findings, a hypothetical model of stress-induced cytoskeletal remodeling is illustrated in Fig. 10.
|
Materials and methods |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and methodsReferences |
|---|
(polyclonal) and HRP-conjugated secondary antibodies were from Santa Cruz Biotechnology, Inc. Monoclonal antibodies against the V5 epitope were from Invitrogen. PP2A (catalytic subunit 
) antibody was from BD Biosciences. ASMase polyclonal antibody has been previously described (Zeidan and Hannun, 2007). Polyclonal ezrin antibody (antibody 1; Millipore) was used for Western blotting. A second ezrin polyclonal antibody (antibody 2; Cell Signaling Technology) was used for immunofluorescence. Anti p-ERM antibody and the second anti-ezrin antibody were purchased from Cell Signaling Technology. AlexaFluor 488, 633, and 546 were from Invitrogen. Okadaic acid and tautomycin were purchased from Calbiochem. Lysenin, cisplatin, bacterial sphingomyelinase derived from Bacillus cereus, and all other materials were from Sigma-Aldrich.
Cell lines and culture conditions
MCF-7 cells were originally purchased from American Type Culture Collection (Manassas, VA). Cells were maintained in RPMI 1640 supplemented with 10% FBS at 37°C in a 5% CO2 incubator. Where indicated, cells were shifted to a phosphate-free medium. Testing for the presence of mycoplasma infections was performed routinely on a monthly basis.
Immunoprecipitation and Western blotting
Cells were treated as indicated in figure legends. Cells were then lysed in a buffer containing 20 mM Tris-HCl, pH 7.5, 100 mM NaCl, 1% NP-40, 2 mM EDTA, 5 mM sodium fluoride, 1.75 mM sodium orthovanadate, 1 mM phenylmethylsulfonyl fluoride, 20 mM β-glycerol phosphate, 10 µg/ml leupeptin, 10 µg/ml aprotinin, and 1 µM microcystin. Homogenates were centrifuged at 3,000 g for 10 min. The supernatants were used for immunoprecipitation using specific monoclonal antibodies (1 µg/ml) overnight. Immune complexes were isolated by incubation with protein G–Agarose beads for 3 h. Western blot analysis was carried using similar procedures as described previously (Zeidan et al., 2006).
SMase assays
In vitro enzymatic assays for acid and neutral sphingomyelinases were performed using [choline-methyl-14C] sphingomyelin. The assays were performed as previously reported (Marchesini et al., 2003; Zeidan et al., 2006).
RNA interference
Gene silencing of human ASMase and PP2A (catalytic subunit) was performed essentially according to a standard protocol (Zeidan et al., 2006). Sequence-specific ASMase siRNA reagents were purchased from QIAGEN. The sequences of ASMase RNAi duplexes were sequence [1]: sense CUC CUU UGG AUG GGC CUG G antisense CCA GGC CCA UCC AAA GGA G, and sequence [2]: sense GGU CUA UUC ACC GCC AUC A antisense UGA UGG CGG UGA AUA GAC C. The PP2A (catalytic subunit ) RNAi was purchased from Santa Cruz Biotechnology, Inc. The specificity of all RNAi sequences was verified by sequence comparison with the human genome database using the NIH Blast program.
Plasmid constructs and subcloning procedures
The V5-ASMase plasmid has been previously described (Zeidan and Hannun, 2007). Full-length ezrin cDNA and ezrin T567D were a gift of Dr. Monique Arpin (INSERM, Paris, France). The full-length cDNAs of ezrin and PP2A (catalytic subunit) were subcloned into pECFP-C1 and p-EYFP-N1 plasmids, respectively. The CFP tag is situated at the N terminus of PP2A, and the YFP tag is situated at the C terminus of ezrin. EcoRI and BamH1 restriction enzymes were used to place the 929-bp PP2A sequence in frame. EcoRI and SalI restriction enzymes were used to place human ezrin 1760 bp in frame. The integrity of the newly developed plasmids was verified by DNA sequencing. For transient overexpression experiments, endotoxin-free plasmids were transfected into MCF-7 cells using Effectene (QIAGEN) according to the manufacturer's recommendations. LacZ and DN-PKC adenoviruses were provided by Dr V. Natarajan (The Johns Hopkins University, Baltimore, MD).
In vitro PKC kinase assay
PKC immune complexes were washed four times with ice-cold kinase buffer (50 mM Tris-HCl, pH 7.5, 50 mM NaCl, 10 mM MgAc, 0.5 mM EGTA, and 0.1 mM DTT). Immunoprecipitates were incubated with the assay buffer consisting of 20 µM ATP, 5 µCi 32P-ATP, 0.2 mg/ml MBP in the presence of 0.2 mg/ml phosphatidylserine and 20 µg/ml DAG. The reaction was carried at 30°C for 15 min and terminated by addition of SDS-PAGE sample buffer. Proteins were separated by electrophoresis, and autoradiography was performed. Samples from each treatment group were tested for equal levels of PKC after immunoprecipitation by Western blotting.
Confocal microscopy
Approximately 5 x 104 cells were seeded into 2-cm poly-L-lysine coated confocal plates (MatTek Corp). After treatment, cells were fixed with 4% paraformaldehyde for 10 min and permeabilized with methanol for 5 min. Blocking was performed in 2.5% FBS solution. Primary antibodies were diluted in a solution of 1.5% FBS/0.15% saponin and incubated for 3 h (1:200 dilution). The samples were then washed with 1.5% FBS solution three times. This was followed by incubation with secondary antibodies for 1 h at room temperature. Samples were stored at 4°C until image acquisition. Images were acquired using a laser-scanning confocal microscope (LSM 510; Carl Zeiss, Inc.). Excitation wavelengths 488, 543, and 633 were used. Images were acquired at the equatorial plane of monolayer cells guided by DRAQ5 (Qbiogene) nuclear stain and processed using LSM 5 Image Browser (Carl Zeiss, Inc.).
Fluorescence resonance energy transfer (FRET) was used to evaluate protein–protein interaction of PP2A and ezrin in the presence or absence of cisplatin. The applied FRET parameters were: excitation for CFP: 458 nm (argon laser), emission: BP (band pass) 475–525 nm, and excitation for YFP: 514 nm (argon laser) emission LP (long pass) 530. MCF-7 cells were co-transfected with CFP-PP2A (catalytic subunit ) and YFP-ezrin using standard protocols and incubated for 24 h. Images were acquired using a laser-scanning microscope (LSM 510-META; Carl Zeiss, Inc.) under sensitized emission settings. Each image consisted of three channels: donor (CFP) channel; acceptor (YFP) channel; and FRET channel (excitation wavelength 458 nm and emission filters LP 530). For each experiment, appropriate controls transfected with either donor alone (CFP-PP2A) or acceptor alone (YFP-ezrin) were prepared. Cells showing similar fluorescence intensity for the donor (CFP) and acceptor (YFP) were selected for analysis. FRET efficiency was determined using the LSM Image Examiner software (Carl Zeiss, Inc.). FRET pictures were normalized for the FRET efficiencies in the respective setting as indicated by the accompanying rainbow scale (FRET efficiency ranges from blue/0 to red/100%).
Preparation of cytosolic/membrane fractions
Cell pellets from the different treatment groups were lysed by sonication in a buffer consisting of 10 mM Hepes, 150 mM NaCl, 1 mM EDTA, pH 7.4, 5 mM sodium fluoride, 1.75 mM sodium orthovanadate, 1 mM phenylmethylsulfonyl fluoride, 20 mM β-glycerol phosphate, 10 µg/ml leupeptin, 10 µg/ml aprotinin, and 1 µM microcystin. Homogenates were cleared of debris by centrifugation at 500 g at 4°C. Samples of the postnuclear supernatants were supplied with sample buffer and corresponded to total cell lysate fractions (T). The membrane fraction (Mb) was obtained by centrifugation at 100,000 g at 4°C for 1 h. The resultant supernatant was denoted as the cytosolic fraction (C).
Mass spectroscopy for ceramide and sphingomyelin
Sphingolipid analysis was performed using Electrospray Ionization/Tandem Mass Spectrometry (ESI-MS/MS) on a Thermo Finnigan TSQ 7000 triple quadrupole mass spectrometer, operating in a multiple reaction monitoring positive ionization mode. This method has been recently described (Bielawski et al., 2006).
Cell wounding and migration assay
5 x 105 MCF-7 cells stably transfected with V5-ASMase or V5-ASMaseS508A were plated in 6-well culture plates in RPMI medium plus 10% FBS. When cultures were 80% confluent, wounding was performed with a 200-µl Eppendorf micropipette tip. Cells were then washed twice with PBS followed by addition of fresh medium supplemented with mitomycin C (0.5 µg/ml) to control for proliferation. Immediately after wounding, cells were inspected under the microscope (Eclipse TE 200; Nikon) (t = 0). Then at 24 and 48 h, cell migration was analyzed by measuring the maximum migration distance of the cell front into the wounded area. Experiments were performed in triplicate and the distance was measured in three fields of each well.
Preparation of adherent plasma membranes
MCF-7 cells were grown on poly-L-lysine coated confocal dishes 2 cm in diameter. Using a syringe with 25-gauge needle, cells were subjected to repeated streams of 5 ml buffer A: pH 7.4, 10 mM Hepes, 50 mM KCl, and 2 mM MgCl2. Membranes were checked by light microscopy, fixed with 4% formaldehyde, and stained with rhodamine-phalloidin.
F-actin/G-actin in vivo assay
The ratio of filamentous actin (F-actin) to globular actin (G-actin) in MCF7 cells was analyzed using an F-actin/G-actin in vivo assay kit (Cytoskeleton, Inc.) based on the manufacturer's protocol. In brief, following indicated treatments cells were lysed with a cell lysis/F-actin stabilization buffer containing 1 mM ATP and protease inhibitor cocktail. Cells were homogenized by 10 passages through a 28.5-gauge insulin syringe and incubated for 10 min at 37°C. Positive control lysates were incubated with 1 µM phalloidin, and negative control lysates were incubated with 10 µM cytochalasin D. The cell lysates were cleared of unbroken cells and cellular debris by 5 min centrifugation at 2,000 rpm (37°C) followed by centrifugation of the supernatant at 100,000 g for 60 min (37°C) to separate F-actin (pellet) from G-actin (supernatant). The supernatants were separated from the pellets and were immediately placed on ice. The pellets were resuspended to the same volume as the supernatants using ice cold Milli-Q water containing 10 µM cytochalasin D and were incubated on ice for 60 min. Samples were then diluted 10-fold in cold Milli-Q water, and equal volumes (20 µl per lane) were resolved by SDS-PAGE and analyzed by Western blotting with an anti-actin antibody provided with the kit. Western blotting was performed as described above.
Statistical analysis
Mann-Whitney or student's t tests were performed between control and treated states and/or between treatment and treatment plus RNAi-mediated inhibition states on a minimum of three independent experiments. A P-value of 0.05 or less is considered as statistically significant and indicated with an asterisk.
Online supplemental material
Fig. S1 demonstrates the effect of cisplatin on membrane-bound F-actin. Fig. S2 shows resistance of ASMaseS508A cells to cisplatin. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200705060/DC1.
|
Acknowledgments |
|---|
This work was supported by the National Cancer Institute grant NCI P01-CA97132 (to Y.A. Hannun). Work at the Lipidomics Core is supported by National Institutes of Health grant C06 RR018823. Y.H. Zeidan is supported in part by the Cystic Fibrosis Research, Inc. New Horizons Fund. R.W. Jenkins is supported by Medical Scientist Training Program grant GM08716.
Submitted: 11 May 2007
Accepted: 25 March 2008
|
References |
|---|
|
TopAbstractIntroductionResultsDiscussionMaterials and methodsReferences |
|---|
Bezombes, C., G. Laurent, and J.P. Jaffrezou. 2003. Implication of raft microdomains in drug induced apoptosis. Curr. Med. Chem. Anti-cancer. Agents. 3:263–270.[CrossRef][Medline]
Bielawski, J., Z.M. Szulc, Y.A. Hannun, and A. Bielawska. 2006. Simultaneous quantitative analysis of bioactive sphingolipids by high-performance liquid chromatography-tandem mass spectrometry. Methods. 39:8
Bijman, M.N., G.P. van Nieuw Amerongen, N. Laurens, V.W. van Hinsbergh, and E. Boven. 2006. Microtubule-targeting agents inhibit angiogenesis at subtoxic concentrations, a process associated with inhibition of Rac1 and Cdc42 activity and changes in the endothelial cytoskeleton. Mol. Cancer Ther. 5:2348–2357.
Bretscher, A., K. Edwards, and R.G. Fehon. 2002. ERM proteins and merlin: integrators at the cell cortex. Nat. Rev. Mol. Cell Biol. 3:586–599.[CrossRef][Medline]
Brown, M.J., R. Nijhara, J.A. Hallam, M. Gignac, K.M. Yamada, S.L. Erlandsen, J. Delon, M. Kruhlak, and S. Shaw. 2003. Chemokine stimulation of human peripheral blood T lymphocytes induces rapid dephosphorylation of ERM proteins, which facilitates loss of microvilli and polarization. Blood. 102:3890–3899.
Calderon, R.O., and G.H. DeVries. 1997. Lipid composition and phospholipid asymmetry of membranes from a Schwann cell line. J. Neurosci. Res. 49:372–380.[CrossRef][Medline]
Chalfant, C.E., K. Kishikawa, M.C. Mumby, C. Kamibayashi, A. Bielawska, and Y.A. Hannun. 1999. Long chain ceramides activate protein phosphatase-1 and protein phosphatase-2A. Activation is stereospecific and regulated by phosphatidic acid. J. Biol. Chem. 274:20313–20317.
Chalfant, C.E., B. Ogretmen, S. Galadari, B.J. Kroesen, B.J. Pettus, and Y.A. Hannun. 2001. FAS activation induces dephosphorylation of SR proteins; dependence on the de novo generation of ceramide and activation of protein phosphatase 1. J. Biol. Chem. 276:44848–44855.
Chalfant, C.E., Z. Szulc, P. Roddy, A. Bielawska, and Y.A. Hannun. 2004. The structural requirements for ceramide activation of serine-threonine protein phosphatases. J. Lipid Res. 45:496–506.
Charruyer, A., S. Grazide, C. Bezombes, S. Muller, G. Laurent, and J.P. Jaffrezou. 2005. UV-C light induces raft-associated acid sphingomyelinase and JNK activation and translocation independently on a nuclear signal. J. Biol. Chem. 280:19196–19204.
Curto, M., and A.I. McClatchey. 2004. Ezrin ... a metastatic detERMinant? Cancer Cell. 5:113–114.[CrossRef][Medline]
Di Bartolomeo, S., and A. Spinedi. 2002. Ordering ceramide-induced cell detachment and apoptosis in human neuroepithelioma. Neurosci. Lett. 334:149–152.[CrossRef][Medline]
Donati, C., and P. Bruni. 2006. Sphingosine 1-phosphate regulates cytoskeleton dynamics: implications in its biological response. Biochim. Biophys. Acta. 1758:2037–2048.[Medline]
Emert-Sedlak, L., S. Shangary, A. Rabinovitz, M.B. Miranda, S.M. Delach, and D.E. Johnson. 2005. Involvement of cathepsin D in chemotherapy-induced cytochrome c release, caspase activation, and cell death. Mol. Cancer Ther. 4:733–742.
Fievet, B.T., A. Gautreau, C. Roy, L. Del Maestro, P. Mangeat, D. Louvard, and M. Arpin. 2004. Phosphoinositide binding and phosphorylation act sequentially in the activation mechanism of ezrin. J. Cell Biol. 164:653–659.
Fievet, B., D. Louvard, and M. Arpin. 2007. ERM proteins in epithelial cell organization and functions. Biochim. Biophys. Acta. 1773:653–660.[Medline]
Gautreau, A., D. Louvard, and M. Arpin. 2000. Morphogenic effects of ezrin require a phosphorylation-induced transition from oligomers to monomers at the plasma membrane. J. Cell Biol. 150:193–203.
Hanada, K., T. Hara, M. Fukasawa, A. Yamaji, M. Umeda, and M. Nishijima. 1998. Mammalian cell mutants resistant to a sphingomyelin-directed cytolysin. Genetic and biochemical evidence for complex formation of the LCB1 protein with the LCB2 protein for serine palmitoyltransferase. J. Biol. Chem. 273:33787–33794.
Heinrich, M., M. Wickel, W. Schneider-Brachert, C. Sandberg, J. Gahr, R. Schwandner, T. Weber, P. Saftig, C. Peters, J. Brunner, et al. 1999. Cathepsin D targeted by acid sphingomyelinase-derived ceramide. EMBO J. 18:5252–5263.[CrossRef][Medline]
Heinrich, M., M. Wickel, S. Winoto-Morbach, W. Schneider-Brachert, T. Weber, J. Brunner, P. Saftig, C. Peters, M. Kronke, and S. Schutze. 2000. Ceramide as an activator lipid of cathepsin D. Adv. Exp. Med. Biol. 477:305–315.[Medline]
Heinrich, M., J. Neumeyer, M. Jakob, C. Hallas, V. Tchikov, S. Winoto-Morbach, M. Wickel, W. Schneider-Brachert, A. Trauzold, A. Hethke, and S. Schutze. 2004. Cathepsin D links TNF-induced acid sphingomyelinase to Bid-mediated caspase-9 and -3 activation. Cell Death Differ. 11:550–563.[CrossRef][Medline]
Herr, I., D. Wilhelm, T. Bohler, P. Angel, and K.M. Debatin. 1997. Activation of CD95 (APO-1/Fas) signaling by ceramide mediates cancer therapy-induced apoptosis. EMBO J. 16:6200–6208.[CrossRef][Medline]
Hu, W., R. Xu, G. Zhang, J. Jin, Z.M. Szulc, J. Bielawski, Y.A. Hannun, L.M. Obeid, and C. Mao. 2005. Golgi fragmentation is associated with ceramide-induced cellular effects. Mol. Biol. Cell. 16:1555–1567.
Kondo, T., K. Takeuchi, Y. Doi, S. Yonemura, S. Nagata, and S. Tsukita. 1997. ERM (ezrin/radixin/moesin)-based molecular mechanism of microvillar breakdown at an early stage of apoptosis. J. Cell Biol. 139:749–758.
Kruidering, M., B. van de Water, Y. Zhan, J.J. Baelde, E. Heer, G.J. Mulder, J.L. Stevens, and J.F. Nagelkerke. 1998. Cisplatin effects on F-actin and matrix proteins precede renal tubular cell detachment and apoptosis in vitro. Cell Death Differ. 5:601–614.[CrossRef][Medline]
Lacour, S., A. Hammann, S. Grazide, D. Lagadic-Gossmann, A. Athias, O. Sergent, G. Laurent, P. Gambert, E. Solary, and M.T. Dimanche-Boitrel. 2004. Cisplatin-induced CD95 redistribution into membrane lipid rafts of HT29 human colon cancer cells. Cancer Res. 64:3593–3598.
Levade, T., and J.P. Jaffrezou. 1999. Signalling sphingomyelinases: which, where, how and why? Biochim. Biophys. Acta. 1438:1–17.[Medline]
Lovat, P.E., F. Di Sano, M. Corazzari, B. Fazi, R.P. Donnorso, A.D. Pearson, A.G. Hall, C.P. Redfern, and M. Piacentini. 2004. Gangliosides link the acidic sphingomyelinase-mediated induction of ceramide to 12-lipoxygenase-dependent apoptosis of neuroblastoma in response to fenretinide. J. Natl. Cancer Inst. 96:1288–1299.
Luciani, F., A. Molinari, F. Lozupone, A. Calcabrini, L. Lugini, A. Stringaro, P. Puddu, G. Arancia, M. Cianfriglia, and S. Fais. 2002. P-glycoprotein-actin association through ERM family proteins: a role in P-glycoprotein function in human cells of lymphoid origin. Blood. 99:641–648.
Maceyka, M., S.G. Payne, S. Milstien, and S. Spiegel. 2002. Sphingosine kinase, sphingosine-1-phosphate, and apoptosis. Biochim. Biophys. Acta. 1585:193–201.[Medline]
Mandic, A., J. Hansson, S. Linder, and M.C. Shoshan. 2003. Cisplatin induces endoplasmic reticulum stress and nucleus-independent apoptotic signaling. J. Biol. Chem. 278:9100–9106.
Marchesini, N., and Y.A. Hannun. 2004. Acid and neutral sphingomyelinases: roles and mechanisms of regulation. Biochem. Cell Biol. 82:27–44.[CrossRef][Medline]
Marchesini, N., C. Luberto, and Y.A. Hannun. 2003. Biochemical properties of mammalian neutral sphingomyelinase 2 and its role in sphingolipid metabolism. J. Biol. Chem. 278:13775–13783.
Meisinger, J., S. Patel, K. Vellody, R. Bergstrom, J. Benefield, Y. Lozano, and M.R. Young. 1997. Protein phosphatase-2A association with microtubules and its role in restricting the invasiveness of human head and neck squamous cell carcinoma cells. Cancer Lett. 111:87–95.[CrossRef][Medline]
Metz, R.J., K. Vellody, S. Patel, R. Bergstrom, J. Meisinger, J. Jackson, M.A. Wright, and M.R. Young. 1996. Vitamin D3 and ceramide reduce the invasion of tumor cells through extracellular matrix components by elevating protein phosphatase-2A. Invasion Metastasis. 16:280–290.[Medline]
Ogretmen, B., and Y.A. Hannun. 2004. Biologically active sphingolipids in cancer pathogenesis and treatment. Nat. Rev. Cancer. 4:604–616.[CrossRef][Medline]
Panigone, S., R. Bergomas, E. Fontanella, A. Prinetti, K. Sandhoff, G.A. Grabowski, and D. Delia. 2001. Up-regulation of prosaposin by the retinoid HPR and its effect on ceramide production and integrin receptors. FASEB J. 15:1475–1477.
Pettus, B.J., C.E. Chalfant, and Y.A. Hannun. 2002. Ceramide in apoptosis: an overview and current perspectives. Biochim. Biophys. Acta. 1585:114–125.[Medline]
Prag, S., M. Parsons, M.D. Keppler, S.M. Ameer-Beg, P. Barber, J. Hunt, A.J. Beavil, R. Calvert, M. Arpin, B. Vojnovic, and T. Ng. 2007. Activated ezrin promotes cell migration through recruitment of the GEF Dbl to lipid rafts and preferential downstream activation of Cdc42. Mol. Biol. Cell. 18:2935–2948.
Prinetti, A., D. Millimaggi, S. D'Ascenzo, M. Clarkson, A. Bettiga, V. Chigorno, S. Sonnino, A. Pavan, and V. Dolo. 2006. Lack of ceramide generation and altered sphingolipid composition are associated with drug resistance in human ovarian carcinoma cells. Biochem. J. 395:311–318.[CrossRef][Medline]
Rahmani, M., E. Reese, Y. Dai, C. Bauer, S.G. Payne, P. Dent, S. Spiegel, and S. Grant. 2005. Coadministration of histone deacetylase inhibitors and perifosine synergistically induces apoptosis in human leukemia cells through Akt and ERK1/2 inactivation and the generation of ceramide and reactive oxygen species. Cancer Res. 65:2422–2432.
Ruvolo, P.P. 2003. Intracellular signal transduction pathways activated by ceramide and its metabolites. Pharmacol. Res. 47:383–392.[CrossRef][Medline]
Safaei, R., K. Katano, B.J. Larson, G. Samimi, A.K. Holzer, W. Naerdemann, M. Tomioka, M. Goodman, and S.B. Howell. 2005. Intracellular localization and trafficking of fluorescein-labeled cisplatin in human ovarian carcinoma cells. Clin. Cancer Res. 11:756–767.
Stover, T.C., A. Sharma, G.P. Robertson, and M. Kester. 2005. Systemic delivery of liposomal short-chain ceramide limits solid tumor growth in murine models of breast adenocarcinoma. Clin. Cancer Res. 11:3465–3474.
Toman, R.E., S.G. Payne, K.R. Watterson, M. Maceyka, N.H. Lee, S. Milstien, J.W. Bigbee, and S. Spiegel. 2004. Differential transactivation of sphingosine-1-phosphate receptors modulates NGF-induced neurite extension. J. Cell Biol. 166:381–392.
van Helvoort, A., M.L. Giudici, M. Thielemans, and G. van Meer. 1997. Transport of sphingomyelin to the cell surface is inhibited by brefeldin A and in mitosis, where C6-NBD-sphingomyelin is translocated across the plasma membrane by a multidrug transporter activity. J. Cell Sci. 110:75–83.[Abstract]
Xu, L., and X. Deng. 2006. Suppression of cancer cell migration and invasion by protein phosphatase 2A through dephosphorylation of mu- and m-calpains. J. Biol. Chem. 281:35567–35575.
Yoshinaga-Ohara, N., A. Takahashi, T. Uchiyama, and M. Sasada. 2002. Spatiotemporal regulation of moesin phosphorylation and rear release by Rho and serine/threonine phosphatase during neutrophil migration. Exp. Cell Res. 278:112–122.[CrossRef][Medline]
Zeidan, Y.H., and Y.A. Hannun. 2007. Activation of acid sphingomyelinase by protein kinase C{delta }-mediated phosphorylation. J. Biol. Chem. 282:11549–11561.
Zeidan, Y.H., B.J. Pettus, S. Elojeimy, T. Taha, L.M. Obeid, T. Kawamori, J.S. Norris, and Y.A. Hannun. 2006. Acid ceramidase but not acid sphingomyelinase is required for tumor necrosis factor-{alpha }-induced PGE2 production. J. Biol. Chem. 281:24695–24703.
CiteULike 
Complore 
Connotea 
Del.icio.us 
Digg 
Reddit 
Technorati What's this?
This article has been cited by other articles:
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
|
|
