O-Glycosylation of Mucin-like Domain Retains the Neutral Ceramidase on the Plasma Membranes as a Type II Integral Membrane Protein*

Motohiro TaniDagger , Hiroshi Iida§, and Makoto ItoDagger

From the Dagger  Department of Bioscience and Biotechnology and the § Department of Applied Genetics and Pest Management, Graduate School of Bioresource and Bioenvironmental Sciences, Kyushu University, 6-10-1 Hakozaki, Higashi-ku, Fukuoka 812-8581, Japan

Received for publication, August 5, 2002, and in revised form, December 20, 2002

    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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DISCUSSION
REFERENCES

Ceramidase is a key enzyme involved in regulating cellular levels of ceramide, sphingosine, and possibly sphigosine 1-phosphate and thus could modulate sphingolipid signaling. Here we report that O-glycosylation of the mucin-like domain of neutral ceramidases was required for localization to the surface of plasma membranes. The deduced amino acid sequences of the mammalian enzymes contain a serine-threonine-rich domain (mucin box), which follows the signal/anchor sequence, whereas those of bacterial and invertebrate enzymes completely lack a mucin box, suggesting that the specific domain has been acquired during evolution. In HEK293 cells overexpressing ceramidase, the enzyme was not only secreted into the medium after cleavage of the NH2-terminal signal/anchor sequence but also localized at the plasma membrane as a type II integral membrane protein. Lectin blot analysis using peanut agglutinin revealed that the mucin box of the enzyme is highly glycosylated with O-glycans. Interestingly, a mutant lacking the mucin box or possible O-glycosylation sites in the mucin box was secreted into the medium but not localized at the surface of the cells. Furthermore, a mucin box-fused chimera green fluorescent protein (GFP), but not GFP itself, with the signal/anchor sequence was distributed on the surface of the cells. These results suggest that O-glycosylation of the mucin box retains proteins on the plasma membranes. We also found that the 112-kDa membrane-bound enzyme from mouse kidney is O-glycosylated, whereas the 94-kDa soluble enzyme from liver is not. These results clearly indicate that post-translational modification of the enzyme with O-glycans is tissue-specific and helps the enzyme to localize at the surface of plasma membranes as a type II membrane protein.

    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Sphingolipids have emerged as a multifunctional lipid biomodulator within or among cells. Ceramide (N-acylsphingosine, Cer),1 a common lipid backbone of sphingomyelin (SM) and glycosphingoslipids, has been shown to mediate many cellular events, including cell growth arrest, differentiation, and apoptosis (1, 2), possibly regulating various cytoplasmic proteins such as protein kinases C-zeta (3), C-alpha , and C-delta (4), and protein phosphatases 1 and 2A (5). Sphingosine (Sph), the N-deacylated product of Cer, exerts mitogenic and apoptosis-inducing activities, depending on the cell type and cell cycle (6, 7). Sph is known to be a potent inhibitor of protein kinase C (8) and an activator of 3-phosphoinositide-dependent kinase 1, which is thought to be occasionally localized at the inner plasma membrane (9). Notably, Sph can be phosphorylated to yield Sph 1-phosphate (S1P), which regulates cell proliferation (10), motility (11), and morphology (12). In contrast to Cer and Sph, S1P appears to act extracellularly by interacting with cell surface G protein-coupled receptors, the endothelial differentiation gene (EDG) family (13).

Ceramidase (CDase, EC 3.5.1.23), an enzyme that catalyzes hydrolysis of the N-acyl linkage of Cer to produce Sph, has been classified into three types mainly based on catalytic pH optima, i.e. acidic, neutral, and alkaline. Neutral CDases, which have an optimum pH of 6.5-8.5, have been cloned from bacteria (14), Drosophila (15), mouse (16), rat (17), and human (18). Interestingly, phylogenetic analysis revealed that the three CDase isoforms having different pH optima may be derived from different ancestral genes (16). Mammalian neutral CDase seems to regulate the balance of Cer/Sph/S1P in response to various stimuli, including cytokines (19, 20) and growth factor (21), and thus could modulate sphingolipid-mediated signaling. Furthermore, the fact that Sph is not produced by de novo synthesis (22) implies a significant role for CDase in the generation of Sph and possibly S1P.

We found that neutral CDases of bacteria (14) and Drosophila (15) were released from cells as a soluble form, whereas those of mammalian origins were mainly recovered in membrane fractions (21). Recently, it was found that the intracellular distribution of the mammalian enzyme was cell/tissue-specific. In rat kidney, neutral CDase was mainly localized at the apical membrane of proximal tubules, distal tubules, and collecting dusts, whereas in liver the enzyme was distributed among endosome-like organelles in hepatocytes (17). Human neutral CDase was exclusively localized to mitochondria in HEK293 and MCF7 cells when overexpressed as a fusion construct with green fluorescent protein (GFP) at the NH2 terminus of the enzyme (18). Furthermore, both neutral and acid CDases were found to be released by murine endothelial cells (23). However, the molecular mechanism by which neutral CDases are localized to different organelles is not well understood.

This report clearly shows that O-glycosylation of the mucin-like domain (mucin box) is required to retain neutral CDases on the plasma membranes as a type II integral membrane protein. It was found that the domain was occasionally lost by post-translational processing, resulting in a different localization of the enzyme. These findings facilitate the understanding of the mechanism for cell/tissue-specific localization of neutral CDases and provide some insight into sphingolipid metabolism at the cell surface or in the extracellular milieu.

    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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Materials-- CHOP cells and anti-Rab6 antibody were kindly provided by Dr. K. Nara (Mitsubishi Kagaku Institute of Life Sciences, Tokyo, Japan) and Dr. S. Tanaka (Shizuoka University, Shizuoka, Japan). HRP-labeled anti-mouse IgG antibody was purchased from Nacalai Tesque (Tokyo, Japan). Cy3-labeled anti-mouse IgG antibody, anti-FLAG M2 antibody, benzyl-GalNAc, brefeldin A, and cytochalasin D were obtained from Sigma. ECL Plus, HRP-labeled, and Cy3-labeled anti-rabbit IgG antibodies were from Amersham Biosciences. Anti-myc and anti-GFP antibodies were purchased from Invitrogen Co. Anti-neutral CDase antibody was raised in a rabbit using the recombinant rat CDase as the antigen (17). C12-NBD-Cer was prepared as described in a previous study (24). HEK293 cells (JCRB9068, established by F. L. Graham) were obtained from the Human Science Research Resource Bank. All other reagents were of the highest purity available.

Plasmid Construction-- The vector pcDNA3.1/Myc-His(+) containing a full-length rat neutral CDase gene (pcDNAkCD) was constructed as described previously (17). To generate a construct expressing the GFP-fused neutral CDase, the vector pcDNAkCD was treated with KpnI and XhoI, and subcloned into pBluescript II SK (Stratagene). The product of the full-length neutral CDase gene digested with KpnI and SmaI was cloned into pEGFP-N2 (Clontech). A mutant, which lacks the mucin-like domain (Delta mucin), was constructed by fusing the NH2-terminal fragment of Met1-Lys42 with the COOH-terminal fragment of Asn79-Thr761. The NH2-terminal fragment was amplified by PCR using a 5' primer with a KpnI restriction site (5'-AGGGTACCGAAATGGCAAAGCGAACCTTCTCC-3') and a 3' primer (5'-ACACCAATGTAGTAGCCACTGAAGTTTTTGTGGTTTTCGATGGTCCC-3'). The COOH- terminal fragment was amplified with a 5' primer (5'-GGGACCATCGAAAACCACAAAAACTTCAGTGGCTACTACATTGGTGT-3') and a 3' primer with an XhoI restriction site (5'-GCCGCTCGAGAGTAGTGACAATTTCAAAAGGGGAAGA-3'). These fragments were extended with Pyrobest DNA polymerase (Takara Shuzo Co.) and subcloned into the vector pcDNA3.1/Myc-His(+) (Invitrogen). To obtain wild-type and Delta mucin CDases tagged with the FLAG epitope (MDYKDDDDK) at the NH2 terminus, DNA fragments of the FLAG-tagged CDases were amplified by PCR using a 5' primer with a KpnI restriction site (5'-AGGTGGTACCATGGACTACAAAGACGATGACGACAAGGCAAAGCGAACCTTCTCCTCC-3') and a 3' primer with an XhoI restriction site (5'-GCCGCTCGAGAGTAGTGACAATTTCAAAAGGGGAAGA-3') and subcloned into the vector pcDNA3.1/Myc-His(+). The mucin box-fused chimera GFP with signal/anchor sequence (S-M-GFP) and GFP with signal/anchor sequence (S-GFP) were designed using the two sequences of the NH2-terminal fragments of the enzyme, Met1-Gln78 and Met1-Lys42, respectively. Each sequence was amplified by PCR using a 5' primer with a KpnI restriction site (5'-AGGGTACCGAAATGGCAAAGCGAACCTTCTCC-3') and a 3' primer with a BamHI restriction site (5'-CCACGGATCCCCTGAGAGGGAGGGAGGTCTGG-3') or (5'-TTCCGGATCCCTTTGTGGTTTTCGATGGTCCC-3'). The amplified fragments were subcloned into pEGFP-N2. Construction of a mutant (Muc-Ala), in which all Ser and Thr residues of mucin box were replaced with Ala residues, is described below. An NH2-terminal fragment (Met1-Pro62) was amplified with a 5' primer with a KpnI restriction site (5'-AGGGTACCGAAATGGCAAAGCGAACCTTCTCC-3'), and a 3' primer (5'-TGGAGCTGCCTGGGCGGCTGCGGGTCCCTGCGCGGCTGCAACCCAATGATTCCCTGCATCTT-3'). A COOH-terminal fragment (Asp43-Asn330) was amplified with a 5' primer (5'-AAGATGCAGGGAATCATTGGGTTGCAGCCGCGCAGGGACCCGCAGCCGCCCAGGCAGCTCCAGCCGCACAAGCTCCAGCCGCACAAGCTCCAGACCTCCCTCCCGCTCAG-3') and a 3' primer (5'-GCAGGCTTTGCTTCATCAA-3'). These fragments were extended with Pyrobest DNA polymerase, digested with KpnI and BamHI, and subcloned into pcDNAkCD. The sequences of these constructs were verified with a DNA sequencer (model 377, Applied Biosystems, Japan).

CDase Assay-- CDase activity was measured using C12-NBD-Cer as a substrate as described in a previous study (25).

Cell Culture and cDNA Transfection-- HEK293 cells, human embryonic kidney cells, were grown in Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% fetal bovine serum (FBS), and 60 µg/ml kanamycin in a humidified incubator containing 5% CO2. CHOP cells, Chinese hamster ovary cells that express polyoma LT antigen, to support the replication of eukaryotic expression vectors (26), were grown in alpha -minimal essential medium (alpha -MEM) supplemented with 10% FBS, 100 µg/ml streptomycin, and 100 units/ml penicillin in a humidified incubator containing 5% CO2. cDNA transfection was carried out using LipofectAMINETM Plus (Invitrogen) according to the instructions of the manufacturer.

Preparation of Culture Supernatants and Cell Lysates-- At 18 h after transfection with the CDase cDNA, the medium was replaced with serum-free Opti-MEM (Invitrogen, 500 µl/well on 24-well plates) and cultured for an additional 24 h. The cell culture medium was collected and subjected to centrifugation at 13,000 × g for 5 min. The supernatant, supplemented with a 1/10 volume of 200 mM Tris-HCl, pH 7.5, containing 1% Triton X-100 and 3.3 µg/ml proteinase inhibitors (leupeptin, pepstatin, and chymostatin), was used as cell supernatant. Cells attached to the culture plate were rinsed with PBS and then lysed by adding 200 µl of 10 mM Tris-HCl, pH 7.5, containing 0.5% Triton X-100 and 3.3 µg/ml of the proteinase inhibitors described above. Lysates were collected by pipette and used as cell lysates.

Protein Assay, SDS-PAGE, and Western Blotting-- Protein content was determined by the bicinchoninic acid protein assay (Pierce) with bovine serum albumin as standard. SDS-PAGE was carried out according to the method of Laemmli (27). Protein transfer onto a polyvinylidene difluoride membrane was performed using Trans-Blot SD (Bio-Rad) according to the method described in a previous study (28). After treatment with 3% skim milk in Tris-buffered saline (TBS) containing 0.1% Tween 20 (T-TBS) for 1 h, the membrane was incubated with primary antibody for 1 day at 4 °C. After a wash with T-TBS, the membrane was incubated with HRP-conjugated secondary antibody for 2 h. After another wash with T-TBS, the ECL reaction was performed for 2-3 min as recommended by the manufacturer, and chemiluminescent signals were visualized on ECLTM Mini-camera (Amersham Biosciences).

Amino Acid Sequencing-- The NH2-terminal sequence of the 94-kDa soluble CDase was determined by the method described previously (25), i.e. the 94-kDa band was visualized by SDS-PAGE with GelCode Blue Stain reagent (Pierce), extracted from the gel, and determined by automated Edman degradation using an amino acid sequencer model 477A (PE Biosystems).

Immunoprecipitation of CDase-- Anti-neutral CDase antibody at a dilution of 1:100 was conjugated with 10 µl of protein A-agarose (Santa Cruz Biotechnology) in 100 µl of reaction buffer (10 mM Tris-HCl, pH 7.5, containing 150 mM NaCl, 1% Triton X-100, and 0.1% bovine serum albumin) at 4 °C for 2 h. After five washes with reaction buffer, 10 µl of protein A-agarose conjugated with antibody was resuspended in 900 µl of reaction buffer, to which 100 µl of denatured CDase was added, and then incubation conducted at 4 °C for 18 h. Before immunoprecipitation, CDase was denatured by boiling for 5 min in 100 µl of SDS sample buffer (20 mM Tris-HCl, pH 7.5 containing 1% SDS and 1% 2-mercaptoethanol). The precipitate was spun down by centrifugation, washed with reaction buffer five times, and then suspended in 20 µl of SDS sample buffer. After boiling at 100 °C for 5 min, the sample was subjected to SDS-PAGE, followed by Western blotting analysis as described above.

Immunocytochemistry and Fluorescence Microscopy-- Transfected cells were cultured on cover glass and then fixed with 3% paraformaldehyde in PBS for 15 min. After being rinsed with PBS and 50 mM NH4Cl in PBS, cells were permeabilized, if necessary, by 0.1% Triton X-100 in PBS. After treatment with blocking buffer (5% skim milk in PBS) for 15 min, the samples were incubated with primary antibody (diluted 1:1000 with blocking buffer) at 4 °C for 1 day followed by Cy3-labeled secondary antibody at room temperature for 2 h. Immunostained samples were examined with a confocal laser-scanning microscope (Digital Eclipse C1, Nikon, Japan).

Flow Cytometric Analysis-- Transfected cells were harvested and incubated with primary antibody (1:1000) in 100 µl of PBS containing 50% FBS on ice for 1.5 h. After being washed twice with PBS, cells were treated with Cy3-labeled secondary antibody in 100 µl of PBS containing 50% FBS on ice for 1 h and then analyzed by flow cytometry (EPICS XL System-IC, Beckman Coulter).

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Subcellular Localization and Topology of Neutral CDase-- The neutral CDase was reported to be localized at apical membranes of rat kidney (17), whereas the enzyme was actively released from murine endothelial cells (23). We found that the CDase fused with GFP at the COOH terminus of the enzyme (Fig. 1E, all constructs used in this study are illustrated in Fig. 1) was distributed in ER/Golgi compartments as well as the plasma membranes of HEK293 cells using a confocal laser microscope (Fig. 2A). The fluorescent signal for GFP-fused CDase was partly co-localized with that for Rab6, a marker protein for Golgi apparatus (Fig. 2B). To clarify the topology of the CDase, a double-tagged CDase, with a FLAG tag at the NH2 terminus and myc tag at the COOH terminus, was constructed (Fig. 1C) and expressed in HEK293 cells. The FLAG signal was observed in ER/Golgi compartments as well as on plasma membranes when cells were permeabilized with Triton X-100 (Fig. 2C, panel a). However, the signal was not detected in intact cells (Fig. 2C, panel b). On the other hand, the COOH-terminal myc signal was observed on plasma membranes with and without treatment of Triton X-100 (Fig. 2C, panels c and d). These results indicate that the COOH terminus of the CDase resides on the extracellular side of the plasma membrane, whereas the NH2 terminus is on the cytoplasmic side. In conclusion, the neutral CDase was expressed on plasma membranes as a type II integral membrane protein in HEK293 cells, being anchored to the membranes with an internal uncleaved NH2-terminal signal/anchor sequence.


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Fig. 1.   Schematic diagram of cDNA constructs. The diagram shows the structures of cDNA constructs used in this study. A, wild-type CDase (wild-type CDase tagged with myc at the COOH terminus); B, Delta mucin CDase (mucin box-deleted mutant CDase tagged with myc at the COOH terminus); C, FLAG-tagged CDase (neutral CDase tagged with FLAG at the NH2 terminus and myc at the COOH terminus); D, FLAG-tagged Delta mucin CDase (mucin box-deleted mutant CDase tagged with FLAG at the NH2 terminus and myc at the COOH terminus); E, GFP-fused CDase (neutral CDase fused with GFP at the COOH terminus); F, S-M-GFP (mucin box with signal/anchor sequence fused with GFP); G, S-GFP (signal/anchor sequence fused with GFP).


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Fig. 2.   Immunocytochemical analysis of the neutral CDase overexpressed in HEK293 cells. A, HEK293 cells overexpressing GFP-fused neutral CDase. Cells were fixed and examined for GFP fluorescence under a confocal laser microscope. Arrows and an arrowhead indicate the expression of CDase at plasma membrane and ER/Golgi compartments, respectively. B, HEK293 cells expressing GFP-fused neutral CDase (left) were fixed, and immunostained with anti-Rab6 antibody followed by anti-rabbit IgG-Cy3 (center). Images were merged (right). An arrow indicates the co-localization of neutral CDase and Rab6, a marker protein for the Golgi apparatus. C, analysis of membrane topology of neutral CDase. a, stained with anti-FLAG antibody after permeabilization with Triton X-100. b, same as a but before treatment with Triton X-100. c, stained with anti-myc antibody after permeabilization with Triton X-100. d, same as c but before treatment with Triton X-100. HEK293 cells were transformed with plasmid vector containing FLAG-tagged CDase cDNA, fixed, and then stained with corresponding antibody before and after treatment with Triton X-100 as described under "Experimental Procedures."

Mucin-like Domain of Mammalian Neutral CDases-- Alignment of the deduced amino acid sequences of rat and mouse neutral CDases with those of Pseudomonas aeruginosa, Mycobacterium tuberculosis, Dictyostelium discoideum, and Drosophila melanogaster neutral CDases, revealed that the rat and mouse enzymes have a Ser/Thr-rich domain (amino acids 43-78) downstream of the NH2-terminal hydrophobic region. The hydrophobic region, which is a putative signal sequence, was observed in all CDases except that from M. tuberculosis. However, the Ser/Thr-rich domains were exclusively observed in CDases from mammals (Fig. 3A), suggesting this domain has been given to the enzyme during evolution. This domain shows a characteristic mucin-type repeating structure that contains not only Ser and Thr but also Pro and Gln and thus was tentatively designated the mucin box in this study. Sequences homologous to the rat and mouse mucin box were found in rat sucrase isomaltase, human MUC2, and insect intestinal mucin peptide (Fig. 3B).


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Fig. 3.   Alignments of deduced amino acid sequences of neutral CDases based on NH2-terminal regions (A) and mucin-like domains (B). The identification of the mucin box was performed by a BLAST search program (43).

Expression and Processing of Wild-type and Mucin Box-deleted CDases-- To investigate the effect of the mucin box on the expression and processing of the enzyme, two constructs were generated; a wild-type CDase, which has the entire sequence of rat neutral CDase, and a deletion mutant (Delta mucin), which lacks the mucin box from the wild-type CDase. Both constructs have a signal/anchor sequence at the NH2 terminus and are tagged with myc at the COOH terminus (Fig. 1, A and B). When the wild-type construct was transfected into HEK293 cells, two protein bands having molecular masses of 113 and 133 kDa on SDS-PAGE were detected in cell lysate after visualization with anti-myc antibody (Fig. 4A). The 113- and 133-kDa proteins seem to be glycosylated with high mannose type N-glycans and high mannose/complex/hybrid type N-glycans, respectively, as reported previously (17), suggesting that they are a developing form in the ER and a mature form in the Golgi apparatus, respectively. A single band of ~105 kDa was detected in cell lysate when the Delta mucin CDase was expressed in HEK293 cells and stained with anti-myc antibody (Fig. 4A). Notably, both wild-type and Delta mucin CDases were secreted into the medium (Fig. 4A). To investigate whether a NH2-terminal signal/anchor sequence was removed by proteolysis, NH2-terminal FLAG-tagged wild-type (Fig. 1C) and Delta mucin (Fig. 1D) CDases were constructed and expressed in HEK293 cells. Both constructs were also tagged with myc at the COOH terminus. Western blotting analysis using anti-FLAG antibody revealed that both overexpressed wild-type and Delta mucin CDases were FLAG-positive in cell lysates, but those in culture media were FLAG-negative (Fig. 4B). On the other hand, myc-positive CDases were detected in both the lysates and culture media of cells overexpressing wild-type and Delta mucin enzymes (Fig. 4B). These results indicate that the NH2-terminal signal/anchor sequence remains intact before secretion, and the enzyme is secreted possibly after cleavage of the signal/anchor sequence, regardless of the presence or absence of mucin box.


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Fig. 4.   Expression, processing, and secretion of wild-type and mucin box-deleted CDases. A, Western blotting of the CDase expressed in HEK293 cells. Cells were transfected with plasmid vector containing wild-type or Delta mucin CDase cDNA. The cell lysates and the culture supernatants were separately subjected to SDS-PAGE (7.5% gels), followed by Western blotting using anti-myc antibody. B, the same experiment was carried out as shown in A, but cells were transfected with plasmid vector containing FLAG-tagged wild-type or Delta mucin CDase cDNA. The cell lysates and the culture supernatants were separately subjected to Western blotting using anti-myc antibody (upper) or anti-FLAG antibody (lower). C and M indicate cell lysate and medium (culture supernatant), respectively.

O-Glycosylation and Secretion of the CDase-- To verify whether or not the mucin box is actually glycosylated with O-glycans, wild-type and Delta mucin CDases were subjected to lectin blotting using peanut agglutinin (PNA), which specifically binds to the Galbeta 1,3GalNAc sequence of O-glycans (29). For wild-type enzyme, the 133-kDa mature form, but not the 113-kDa ER form, was stained with the lectin, whereas no band was stained for Delta mucin CDase (Fig. 5A). Furthermore, treatment of CDase-overexpressing cells with benzyl-GalNAc, an inhibitor of O-glycosylation, resulted in a reduction in the molecular mass of the 133-kDa, but not the 113-kDa, wild-type CDase. The inhibitor did not affect the molecular mass of the Delta mucin CDase (Fig. 5B). These results suggest that O-glycosylation crucially occurred in the mucin box of the CDase possibly at the Golgi apparatus. The secreted wild-type CDase was also stained with PNA (data not shown), suggesting that the mucin box is not removed by proteolytic processing of the signal/anchor sequence in HEK293 cells. The wild-type as well as Delta mucin CDase was continuously released from cells into the culture medium (Fig. 6A). It should be noted, however, that the Delta mucin CDase was found to be secreted much faster than the wild-type enzyme. The secretion of both enzymes was strongly inhibited by brefeldin A and treatment at 5 °C but not by cytochalasin D (Fig. 6B), suggesting that the two CDases were processed and secreted by a pathway via ER/Golgi compartments.


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Fig. 5.   O-Gylcosylation of neutral CDase. A, lectin blotting of wild-type and mucin box-deleted CDases. The lysates of HEK293 cells transfected with plasmid vector containing wild-type or Delta mucin CDase cDNA were subjected to immunoprecipitation using anti-neutral CDase antibody as described under "Experimental Procedures." Thereafter, the immunoprecipitants were subjected to SDS-PAGE, followed by Western blotting using anti-myc antibody or lectin blotting using HRP-labeled PNA. B, inhibition of O-glycosylation by benzyl-GalNAc. At 4 h after transfection, the cells were treated with or without 5 mM benzyl-GalNAc in DMEM supplemented with 10% FBS and then cultured for an additional 20 h. Cells were lysed and subjected to SDS-PAGE, followed by Western blotting using anti-myc antibody.


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Fig. 6.   Secretion of wild-type and mucin box-deleted CDases. A, time course for the secretion of wild-type and Delta mucin CDases. At 18 h after transfection, the medium was replaced with serum-free Opti-MEM and the cells were incubated at 37 °C for the period indicated. The culture supernatant was employed for the determination of neutral CDase activity using C12-NBD-Cer as a substrate and Western blotting with anti-myc antibody. B, effects of brefeldin A (BFA), cytochalasin D (CytoD), and temperature on the secretion of CDase. At 18 h after transfection, cells were incubated with 10 µg/ml BFA or 5 µM CytoD in DMEM supplemented with 10% FBS at 37 °C for 1 h. The medium was replaced with Opti-MEM containing the inhibitors at the same concentrations and then cultured at 37 °C for an additional 3 h. To examine the effect of temperature, transfected cells were incubated at 5 °C for 3 h in fresh Opti-MEM without inhibitors.

Mucin Box-mediated Cell Surface Expression of Neutral CDase-- To investigate the role of the mucin box in the subcellular localization of the neutral CDase, immunocytochemical analysis of wild-type and Delta mucin CDases (Fig. 1, A and B), both of which were tagged with myc at the COOH terminus, was performed. Interestingly, the myc signal of the wild-type CDase was much stronger than that of the Delta mucin CDase when the transformed cells were not permeabilized (Fig. 7A, panels a versus c), although the expression levels of the enzymes were almost the same when cells were permeabilized with Triton X-100 (Fig. 7A, panels b versus d). Flow cytometric analysis also showed a clear difference in the cell surface expression of myc signal of the enzyme due to the presence of a mucin box, i.e. wild-type CDase localized at the surface of plasma membranes of HEK293 as well as CHOP cells but Delta mucin enzyme did not (Fig. 7, B and C).


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Fig. 7.   Cell surface expression of neutral CDase. A, expression of neutral CDase on the surface (a and c) or inside (b and d). Wild-type- (a and b) and Delta mucin-expressing HEK293 cells (c and d) were fixed, permeabilized by Triton X-100 (b and d) or not (a and c), and stained with anti-myc antibody. B and C, cell surface expression of neutral CDase in HEK293 (B) and CHOP (C) cells. Cells (3 × 105) were transfected with plasmid vector containing wild-type or Delta mucin CDase cDNA, or empty vector (Mock) and then cultured at 37 °C for 24 h. Cells were harvested and incubated with anti-myc antibody followed by anti-mouse IgG-Cy3 at 4 °C and analyzed by flow cytometry as described under "Experimental Procedures."

Significance of O-Glycosylation in the Mucin Box for Cell Surface Expression of the CDase-- It was revealed by lectin blotting that the mucin box of the CDase was actually glycosylated with O-glycans (Fig. 5). To investigate the significance of O-glycans in the mucin box for cell surface expression of the CDase, the possible O-glycosylation sites (all Ser and Thr residues) of the mucin box were mutated with Ala (Fig. 8A). When the mutant CDase (Muc-Ala) was transfected into CHOP cells, a single protein band showing 113 kDa was detected in the cell lysate. In contrast to the 133-kDa Golgi form of the wild-type CDase, the Muc-Ala 113 kDa band was not affected when the benzyl-GalNAc, an inhibitor for O-glycosylation, was added into the culture of CHOP cells, indicating the mutant lost the O-glycans as expected (Fig. 8B). Although both wild-type and Muc-Ala mutant CDases were continuously released into the culture medium, the amount of secreted enzyme was significantly increased by the removal of O-glycans from the mucin box (Fig. 8C). In contrast, the cell surface expression of the enzyme was markedly reduced by removal of O-glycans (Fig. 8D, panels a versus c). It is noted, however, that the expression of the mutant CDase was almost the same as that of wild-type CDase (Fig. 8D, panels b versus d). Taken together, it was concluded that the O-glycosylation of the mucin box of the CDase helps the enzyme to localize at the surface of plasma membranes as a type II integral membrane protein.


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Fig. 8.   Effects of mutation of possible O-glycosylation sites on the secretion and cell surface expression of the CDase. A, the deduced amino acid sequences of the mucin box in a wild-type CDase and a mutant enzyme disrupting potential O-glycosylation sites (Muc-Ala). All underlined Ser and Thr residues were replaced by Ala as described under "Experimental Procedures." B, Western blotting of wild-type and Muc-Ala CDases expressed in CHOP cells. At 4 h after transfection with plasmid vector containing wild-type or Muc-Ala CDase cDNA, the cells were treated with (+) or without (-) 5 mM benzyl-GalNAc in alpha -MEM supplemented with 10% FBS, and then cultured for an additional 20 h. Cell lysates were subjected to SDS-PAGE, followed by Western blotting using anti-myc antibody. C, time course for the secretion of wild-type and Muc-Ala mutant CDases in CHOP cells. At 18 h after transfection, the medium was replaced with serum-free Opti-MEM, and the cells were incubated at 37 °C for the period indicated. The culture supernatants were employed for the determination of neutral CDase activity using C12-NBD-Cer as a substrate and Western blotting using anti-myc antibody. D, expression of neutral CDase on the surface (a and c) or inside (b and d) of CHOP cells. Cells expressing wild-type (a and b) and Muc-Ala (c and d) CDases were fixed, permeabilized with Triton X-100 (b and d) or not (a and c), and stained with anti-myc antibody. The arrows indicate the expression of CDase at plasma membrane.

Localization of Mucin Box-fused GFP-- To verify the potential role of the mucin box per se, GFP was used as a reporting molecule, i.e. a mucin box-fused chimera with signal/anchor sequence (S-M-GFP) was constructed (Fig. 1F) and expressed in HEK293 cells. Two major bands of 38 and 57 kDa were detected in cell lysates by Western blotting using anti-GFP antibody (Fig. 9A, lane 3). The 57-kDa, but not the 38-kDa, protein was reduced in its molecular mass by treatment with benzyl-GalNAc (data not shown), indicating it was O-glycosylated. The fused protein was found to distribute on the surface of HEK293 cells when stained with anti-GFP antibody (Fig. 9B, panel b). In contrast, GFP with signal/anchor sequence (S-GFP, Fig. 1G) was not expressed on the cell surface (Fig. 9B, panel d), although the intracellular expression of S-GFP was comparable to that of S-M-GFP (Fig. 9B, panels a versus c). Flow cytometric analysis using anti-GFP antibody also revealed that the cell surface signal of S-M-GFP was much stronger than that of S-GFP and mock transfectants when expressed in HEK293 cells (Fig. 9C). These results clearly indicate that the O-glycosylated mucin box functions as a potential signal to retain proteins on the cell surface.


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Fig. 9.   Expression of mucin box-fused GFP. A, SDS-PAGE of the expressed proteins. HEK293 cells were transfected with plasmid vector containing GFP (pEGFP-N2), S-GFP, or S-M-GFP cDNA. Cell lysates were subjected to SDS-PAGE (12.5% gels), followed by Western blotting using anti-GFP antibody. Lane 1, GFP; lane 2, S-GFP; lane 3, S-M-GFP. B, immunocytochemical analysis of S-M-GFP and S-GFP. HEK293 cells overexpressing S-M-GFP (a and b) or S-GFP (c and d) were fixed, and stained with anti-GFP antibody (b and d). The panels a and c show direct GFP fluorescence. C, flow cytometric analysis of cell-surface GFP. HEK293 cells (3 × 105) were transfected with plasmid vector containing GFP (pEGFP-N2), S-GFP, or S-M-GFP cDNA. At 24 h after transfection, cells were harvested, stained with anti-GFP antibody before a second incubation with anti-rabbit IgG-Cy3 at 4 °C, and analyzed by flow cytometry.

Mucin Box in Neutral CDases from Mouse Tissues and Serum-- It was found that in mouse liver 72% of neutral CDase activity was recovered in the soluble fraction after freeze-thawing, whereas in mouse kidney more than 90% of the activity was recovered in the insoluble fraction (Fig. 10A). The neutral CDase in the kidney insoluble fraction was identified as a 112-kDa protein and that in the liver-soluble fraction as a 94-kDa protein by Western blotting using anti-neutral CDase antibody (Fig. 10B). The 112-kDa CDase was also detected in the insoluble fraction of liver (Fig. 10B). Interestingly, the 112-kDa insoluble CDases from kidney and liver were stained by PNA lectin, whereas the 94-kDa soluble CDase was not, indicating that only the CDases in the insoluble fraction were modified with O-glycans. The NH2-terminal sequence of the 94-kDa soluble CDase was determined by the method described in a previous report (25). The determined NH2-terminal sequence corresponded to FSGYYIGVGRADCTGQVSDIN in the deduced sequence (80-100 in Fig. 3A), indicating that the protein does not possess a signal/anchor sequence or a mucin box. Although the insoluble CDases from both liver and kidney were O-glycosylated, the O-glycan structure of kidney CDase seems to be somewhat different from that of the liver enzyme. This is because sialidase treatment significantly reduced the molecular mass and increased the PNA reactivity of the liver CDase but had little effect on the kidney enzyme (Fig. 10B). Furthermore, we found that the PNA-positive CDase was also present in mouse serum, which was possibly derived from liver, because sialidase treatment of the enzyme reduced its molecular mass and increased its PNA reactivity as in the liver CDase (Fig. 10B). These results strongly suggested that post-translational modification of the enzyme with O-glycans is performed in a tissue-specific manner and affects the intracellular distribution of the CDase.


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Fig. 10.   Mucin box in neutral CDases from mouse tissues and serum. A, solubilization by freeze-thawing of neutral CDase from mouse liver and kidney. The preparation of the membrane fraction and solubilization of the neutral CDase by freeze-thawing were performed according to the method described in Ref. 25. Values are the means for duplicate determinations. B, Western and lectin blotting of neutral CDase. Each sample was immunoprecipitated and analyzed by Western blotting using anti-neutral CDase antibody or lectin blotting using HRP-labeled PNA. For sialidase treatment, the immunoprecipitants were detached from agarose beads by addition of 10 µl of 100 mM glycine, pH 2.5. The pH of samples was adjusted to 5.0 by addition of 500 mM sodium acetate buffer, pH 5.0, containing 5 mM CaCl2 and 0.1% Triton X-100. The mixtures were incubated with or without 5 milliunits of sialidase (Vibrio cholera) at 37 °C for 18 h.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

This study demonstrated that the neutral CDase is sorted by a classic pathway via ER/Golgi compartments to the plasma membranes where it is expressed as a type II integral membrane protein or alternatively secreted out of cells after proteolytic processing of the NH2-terminal signal/anchor sequence. This report also clearly indicates that the fate of the protein (as a membrane protein or secretion protein) depends on the presence of a mucin box located in the NH2-terminal region of the enzyme. Because, in contrast to the wild-type CDase, the mucin box-deleted mutant CDase does not localize at the surface of cells and is almost entirely secreted. Furthermore, the fact that bacterial and invertebrate neutral CDases, which lack the mucin box, are secreted without cell surface expression may support this conclusion. In conclusion, the mucin box acquired by the process of evolution enables the mammalian CDase to localize on the cell surface as a type II integral membrane protein. It should be emphasized that the mucin box-mediated cell surface localization is not limited to the neutral CDase but occurs in general, because the mucin box-fused chimeric GFP, but not GFP itself, with signal/anchor sequence was found to be exclusively localized at the surfaces of HEK293 cells.

The mechanism by which the mucin box retains CDase on the cell surface is unclear at present. However, the finding made here that replacement of possible O-glycosylation sites (Ser/Thr residues) with Ala greatly increased the secretion and reduced the expression of the CDase on plasma membranes may indicate specific functions of O-glycans, although the structures of O-glycans remain to be elucidated.

A diverse range of membrane proteins of type I or type II topology are occasionally released from the lipid bilayer by proteolysis catalyzed by a group of enzymes referred to as secretases (30). The proteolytic processing of membrane-bound proteins by secretases is well characterized in amyloid precursor protein (31), a type I integral membrane protein, and a Golgi-resident sialyltransferase (32), a type II integral membrane protein. The latter is cleaved in its membrane-anchoring region by beta -secretase and secreted out of the cell (32). Thus, it is possible that the neutral CDase is detached from cells after processing of the NH2-terminal signal/anchor sequence by secretases. We indicate the possibility that the mucin box interferes with the action of secretases resulting in the generation of the type II membrane-bound CDase, because the mucin box exists very close to the possible cleavage site of the signal/anchor sequence. However, the molecular mechanism for proteolytic processing of the CDase, including the participation of secretases, remains to be clarified. Another possibility is that the mucin box is a potential signal for the sorting of proteins to plasma membranes without processing of the signal/anchor sequence, although the counterparts for the recognition of O-glycans have yet been characterized.

There have been few reports on the role of the O-glycosylation of secretory proteins. It has been reported that O-glycosylation of the COOH-terminal tandem-repeated sequences regulates the secretion of rat pancreatic bile salt-dependent lipase. The O-glycosylation of the enzyme concealed the Pro-, Glu-, Ser-, and Thr-rich domain (PEST region), which is commonly present in rapidly degraded proteins, resulting in delivery to a secretion instead of a degradation pathway (33). In polarized cells, the O-glycosylation was also found to be required for apical sorting of sucrase isomaltase (34) and the neurotrophin receptor (35). It was also reported that a mucin-like domain of enteropeptidase directs apical targeting in Madin-Darby canine kidney cells (36). The neutral CDase was localized at the apical membranes of proximal tubules, distal tubules, and collecting ducts in rat kidney (17) and thus the possible functions of O-glycans in apical sorting should be examined in this CDase.

In contrast to our observation, human neutral CDase has been reported to be expressed in mitochondria when overexpressed in HEK293 and MCF7 cells (18). We found that the deduced NH2-terminal sequence of the human CDase lacks 19 amino acid residues in comparison with those of mouse and rat CDases (16-18). This may result in the generation of an incomplete signal/anchor sequence for ER targeting, allowing the human CDase to target mitochondria instead of the lumen side of the ER.

Recently, evidence has emerged that the outer leaflet of the plasma membrane is a site of SM metabolism; SM is abundant here particularly in lipid microdomain rafts (37), and sphingomyelinase as well as CDase is actively secreted from endothelial cells (23, 38). Furthermore, acid sphingomyelinase was reported to be secreted and helped to metabolize SM in oxidized lipoproteins (39), and CD95 induces the translocation of acid sphingomyelinase onto the cell surface, resulting in the generation of extracellularly orientated Cer (40). The neutral CDase is expressed at the plasma membrane as a type II membrane protein, the catalytic domain of which is located on the extracellular side, or is secreted out of the cell. Importantly, the generation of S1P in the extracellular milieu, which occurs due to the export of the Sph kinase, was reported (41). Very recently, it was found that phorbol 12-myristate 13-acetate induced the protein kinase C-dependent translocation of Sph kinase to the plasma membrane, resulting in the extracellular release of S1P (42). Taken together, all metabolic enzymes required for hydrolysis of SM to generate S1P could be present at the outer leaflet of the plasma membrane or in extra milieu, allowing for the formation of an alternative pathway from SM to S1P. In this context, it is important to note that the neutral CDase was actually detected in mouse serum, which may indicate an important role in vascular biology, i.e. regulating the extracellular content of Cer, Sph, and possibly S1P, all of which may function in autocrine/paracrine signaling.

    ACKNOWLEDGEMENTS

We are grateful to Dr. J. W. Dennis and Dr. K. Nara for the gift of CHOP cells. We also thank Dr. S. Tanaka for the gift of anti-Rab6 antibody. Thanks are also due to Dr. N. Okino and H. Monjusho in our laboratory for supplying the sequence data of the slime mold CDase.

    FOOTNOTES

* This work was supported by a Grant-in-Aid for Scientific Research on Priority Areas (B) 12140204 and Special Coordination Funds for Promoting Science and Technology from the Ministry of Education, Culture, Sports, Science and Technology, Japan.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. Tel.: 81-92-642-2900; Fax: 81-92-642-2907; E-mail: makotoi@agr.kyushu-u.ac.jp.

Published, JBC Papers in Press, December 23, 2002, DOI 10.1074/jbc.M207932200

    ABBREVIATIONS

The abbreviations used are: Cer, ceramide; CDase, ceramidase; FBS, fetal bovine serum; GFP, green fluorescent protein; HRP, horseradish peroxidase; NBD, 4-nitrobenzo-2-oxa-1,3-diazole; PBS, phosphate-buffered saline; PNA, peanut agglutinin; SM, sphingomyelin; Sph, sphingosine; S1P, sphingosine 1-phosphate; CHOP cells, Chinese hamster ovary cells that express polyoma LT antigen; DMEM, Dulbecco's modified Eagle's medium; ER, endoplasmic reticulum.

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DISCUSSION
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