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J. Biol. Chem., Vol. 282, Issue 23, 17024-17031, June 8, 2007

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O-Fucosylation of Thrombospondin Type 1 Repeats in ADAMTS-like-1/Punctin-1 Regulates Secretion

IMPLICATIONS FOR THE ADAMTS SUPERFAMILY^*

Lauren W. Wang, Malgosia Dlugosz, Robert P. T. Somerville, Mona Raed, Robert S. Haltiwanger, and Suneel S. Apte¹

From the Department of Biomedical Engineering, Lerner Research Institute, Cleveland Clinic Foundation, Cleveland, Ohio 44195 and the Department of Biochemistry and Cell Biology, Stony Brook University, Stony Brook, New York 11794-5215

Received for publication, February 5, 2007 , and in revised form, March 29, 2007.

	ABSTRACT

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
The ADAMTS superfamily contains several metalloproteases (ADAMTS proteases) as well as ADAMTS-like molecules that lack proteolytic activity. Their common feature is the presence of one or more thrombospondin type-1 repeats (TSRs) within a characteristic modular organization. ADAMTS like-1/punctin-1 has four TSRs. Previously, O-fucosylation on Ser or Thr mediated by the endoplasmic reticulum-localized enzyme protein-O-fucosyltransferase 2 (POFUT2) was described for TSRs of thrombospondin-1, properdin, and F-spondin within the sequence Cys-Xaa¹-Xaa²-(Ser/Thr)-Cys-Xaa-Xaa-Gly (where the fucosylated residue is underlined). On mass spectrometric analysis of tryptic peptides from recombinant secreted human punctin-1, the appropriate peptides from TSR2, TSR3, and TSR4 were found to bear either a fucose monosaccharide (TSR3, TSR4) or a fucose-glucose disaccharide (TSR2, TSR3, TSR4). Although mass spectral analysis did not unambiguously identify the relevant peptide from TSR1, metabolic labeling of cells expressing TSR1 and the cysteine-rich module led to incorporation of [³H]fucose into this construct. Mutation of the putative modified Ser/Thr residues in TSR2, TSR3, and TSR4 led to significantly decreased levels of secreted punctin-1. Similarly, expression of punctin-1 in Lec-13 cells that are deficient in conversion of GDP-mannose to GDP-fucose substantially decreased the levels of secreted protein, which were restored upon culture in the presence of exogenous L-fucose. In addition, mutation of the single N-linked oligosaccharide in punctin-1 led to decreased levels of secreted punctin-1. Taken together, the data define a critical role for N-glycosylation and O-fucosylation in the biosynthesis of punctin-1. From a broad perspective, these data suggest that O-fucosylation may be a widespread post-translational modification in members of the ADAMTS superfamily with possible regulatory consequences.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
In humans, the ADAMTS superfamily contains 19 ADAMTS proteases and at least five ADAMTS-like proteins. ADAMTS proteases consist of a metalloprotease zymogen domain attached to a C-terminal ancillary domain. The modular construction of the ancillary domain, which includes one or more thrombospondin-type 1 repeats (TSRs),² is a hallmark of the ADAMTS superfamily (1, 2). TSRs were initially discovered in the matricellular protein thrombospondin-1 (3) and were subsequently identified in several other molecules. ADAMTS-like proteins closely resemble the ancillary domains of ADAMTS proteases in their modular content (including the presence of TSRs) and primary sequence but lack the metalloprotease domain, and thus, do not have protease activity (4, 5). ADAMTS-like proteins are not alternatively spliced variants arising from ADAMTS genes, but they are the products of distinct genes. They are present in chordates as well as non-chordates (6), implying conserved functions, although these are presently unknown. Currently, it is considered that some ADAMTS-like proteins may be extracellular matrix components, although a potential regulatory role vis à vis ADAMTS proteases is also supported (4, 5, 7, 8).

ADAMTS-like 1 (ADAMTSL1, also known as punctin-1), the focus of this investigation, is one of a pair of closely related molecules (the other being ADAMTSL3/punctin-2), which are secreted glycoproteins having an affinity for extracellular matrix (4, 5). Although its function is unknown, we have been interested in it as a structural and biochemical model for the ancillary domain of the ADAMTS proteases. Here, we specifically investigated the post-translational modification of punctin-1 by O-fucosylation of its TSRs. Punctin-1 is particularly well suited for such analysis since it contains four TSRs (Fig. 1A), yet it is relatively small (60 kDa) when compared with ADAMTS proteases bearing the same number of TSRs, which facilitates its purification as a recombinant protein (4). Like other members of the superfamily, its TSRs range from 50 to 60 amino acids in length and contain 6 conserved cysteines (4). Punctin-1 has four consensus sites for O-fucosylation and one site for N-linked oligosaccharide attachment, but it lacks predicted sites for mucin-type O-linked oligosaccharide attachment (Fig. 1A) (4).

View larger version (36K): [in this window] [in a new window]   FIGURE 1. Purification of punctin-1 from HEK293F cells and analysis of N-linked glycosylation. A, domain structure of punctin-1 with the key to the various modules shown in the box at right. The O-fucosylation consensus sequences within each TSR are shown at the top, and the putative modified residues are underlined. B, silver staining of purified punctin under reducing (R) and non-reducing (NR) conditions (left-hand panel) and Western blotting (IB) with anti-Myc following treatment with or without peptide-N-glycanase F (PNGase F, right-hand panel). Punctin-1 migrated more rapidly under non-reducing conditions and following removal of its N-linked oligosaccharide. C, expression of wild-type (WT) and N251Q-substituted punctin-1 (NQ) in HEK293F, Cos-1, and CHO-K1 cells and of wild-type punctin-1 in Lec1 cells. The molecular species encoding punctin-1 and IgG (as a control for transfection and secretion efficiency) are indicated. Note the reduced levels of N251Q-substituted punctin-1 in the medium from HEK293F, COS-1, and CHO-K1 cells relative to the wild-type punctin-1 and reduced levels of wild-type punctin in medium from Lec1 cells relative to CHO-K1 cells.

Analysis of fucosylated peptides from thrombospondin-1, F-spondin, and properdin suggested a consensus sequence within each substrate, i.e. Cys¹-Xaa_(2/3)-(Ser/Thr)-Cys²-Xaa₂-Gly (where Cys¹ and Cys² are the 1st and 2nd conserved Cys residue in the TSR) and identified a Ser or Thr residue within this consensus sequence (underlined) as the recipient amino acid for O-fucosylation (16). The high prevalence of this specific modification in the TSRs of these proteins (16) suggested that it could also be present in other TSR-containing proteins, such as of the ADAMTS superfamily. The ADAMTS superfamily contains over 150 TSRs in humans, more than any other class of molecules, suggesting that it could collectively be the major class of substrates for POFUT2. Several members of the ADAMTS superfamily have been implicated in inherited or acquired human disorders: ADAMTS2 in dermatosparaxis, an inherited skin fragility (25), ADAMTS4 and ADAMTS5 in arthritis (26–28), ADAMTS10 in Weill-Marchesani syndrome (29), which is a hereditary generalized mesodermal dysplasia, and ADAMTS13 in thrombocytopenic purpura (30). In addition, critical biological roles for ADAMTS1 and ADAMTS20 have been established in engineered and natural mouse mutants, respectively (31–33). Because of this high biomedical significance, the general molecular features, including post-translational modification, as well as the regulatory and operational mechanisms of this superfamily are of considerable interest.

Whether or not O-fucosylation of TSRs occurs in the ADAMTS superfamily, and its functional significance is hitherto unknown, although every ADAMTS member carries at least one TSR containing the appropriate consensus sequence. Here we have investigated the occurrence and functional relevance of TSR O-fucosylation in the ADAMTS superfamily using punctin-1 as the principal model. The results demonstrate a significant role for O-fucosylation of TSRs as well as N-glycosylation in mediating the efficient secretion of punctin-1 and are thus of broad potential significance for the ADAMTS superfamily.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Plasmid Constructs And Site-directed Mutagenesis—The cDNA plasmid for expression of human punctin-1 with a C-terminal tandem Myc and His₆ tag was previously described (4). Mutations of specific amino acids (N251Q, T312A, S391A, and T451A) were introduced in punctin-1 using the QuikChange site-directed mutagenesis kit (Stratagene, La Jolla, CA). Primers used for mutagenesis are available upon request. A truncated protein construct (TSR1-CRD) containing only TSR1 and the cysteine-rich domain (CRD) was generated by PCR using the full-length punctin-1 construct as template, and the sequence was verified and cloned into pFLAG-CMV-5c (Sigma-Aldrich) for expression with a C-terminal FLAG tag. Wild-type, truncated, and mutant plasmids were expressed in the various cell lines described below.

Cell Culture and Transfections—HEK293F, COS-1, CHO, and Lec1 cells were obtained from ATCC (Manassas, VA) and were routinely maintained as described previously (4, 34). Lec1 cells are CHO derivatives that are deficient in the activity of the Golgi enzyme N-acetylglucosaminyltransferase I (GlcNAc-TI), which is required for the synthesis of hybrid and complex-type N-linked oligosaccharides (35, 36). Since the catalytic step mediated by this enzyme is a prerequisite for the addition of fucose to N-linked oligosaccharides, Lec1 cells incorporate fucose at sites of O-fucosylation but not N-glycosylation (37). Lec1 cells can, however, modify proteins with a simple oligomannose-type N-linked oligosaccharide (37). Lec13 cells (kindly provided by Dr. Pamela Stanley, Albert Einstein College of Medicine, New York, NY) are CHO derivatives that are deficient in the conversion of GDP-mannose to GDP-fucose because of a mutation in GDP-mannose 4,6-dehydratase (34). Thus, they are entirely reliant on L-fucose in conditioned medium (the scavenger pathway) for incorporation of fucose in target oligosaccharides. Subconfluent cells were transiently transfected with the respective plasmids using FuGENE 6 (Roche Diagnostics) as per the manufacturer's recommendation. As an internal control to normalize transfection and secretion efficiency, cells were co-transfected with a plasmid (HIgG-pRK5) encoding the Fc portion of human IgG (kindly provided by Dr. Jen-Chih Hsieh) (38), which lacks any consensus sites for O-fucosylation. To study the effect of O-fucosylation on punctin-1, transfected Lec13 cells were depleted of their fucose stores by culture in medium lacking L-fucose for 5 days prior to transfection. In parallel experiments to permit O-fucosylation, culture was done in medium supplemented with 1 mM L-fucose (Sigma-Aldrich). For production of recombinant punctin-1, HEK293F cells were transfected as above, and stably selected clones were identified and propagated essentially as described previously (39).

Deglycosylation, SDS-PAGE, and Western Blotting—Removal of N-linked oligosaccharide of punctin-1 using peptide-N-glycanase F (Sigma-Aldrich) was done following denaturation as described previously (4). Punctin-1 was detected by Western blotting after reducing SDS-PAGE using anti-Myc monoclonal antibody 9E10 (Invitrogen) or anti-FLAG polyclonal antibody (Sigma-Aldrich). IgG was detected on Western blots using horseradish peroxidase-conjugated goat anti-human IgG (Jackson ImmunoResearch Laboratories, West Grove, PA). For normalization of cellular levels of punctin-1, Western blotting of cell lysate was done using both anti-Myc monoclonal antibody and anti-glyceraldehyde-3 phosphate dehydrogenase (anti-GAPDH, Chemicon, Temecula, CA). To detect binding of these antibodies, we used the appropriate horseradish peroxidase-conjugated secondary antibody and enhanced chemiluminescence (ECL, Amersham Biosciences). Signal intensity of the relevant bands from ECL films was quantitated using ImageJ software (National Institutes of Health, Bethesda, MD). Ratios of signal intensity of the punctin band to the signal intensity of human IgG (conditioned medium) or GAPDH (cell lysates) on the same gel were obtained for comparison of the levels of secreted and intracellular protein, respectively. Statistical analysis was done using the Student's t test.

Metabolic Labeling, Affinity Purification, and Fluorography—Metabolic labeling with [³H]fucose was done essentially as described by Nita-Lazar and Haltiwanger (40). HEK293F cells were cultured in 6-well plates containing 2 ml of Dulbecco's modified Eagle's medium supplemented with 10% fetal bovine serum/well. They were transfected with full-length punctin-1 or TSR1-CRD plasmids when 60% confluent. 16 h following transfection, the medium was changed to 1 ml of serum-free Dulbecco's modified Eagle's medium containing 10 µCi/ml L-[6-³H]fucose (American Radiolabeled Chemicals, St. Louis, MO), and cells were incubated for a further 48 h and then washed three times with phosphate-buffered saline. 100 µl of cell culture lysis reagent (Promega Corp, Madison, WI) with Complete protease inhibitor mixture (Roche Diagnostics) was added to the wells. FLAG-tagged proteins were affinity-purified from the cell lysates using EZ-View Red anti-FLAG M2 affinity gel as per the manufacturer's protocol (30 µl gel/100 µl lysate, Sigma-Aldrich). Untransfected metabolically labeled cells were processed similarly as a negative control. Bound proteins were eluted by boiling, electrophoresed by reducing SDS-PAGE, and detected either by Western blotting using an anti-FLAG polyclonal antibody (Sigma-Aldrich) or by fluorography. For fluorography, eluted proteins were electrophoresed by reducing SDS-PAGE. The gel was soaked in Enlightening^TM rapid autoradiography enhancer (PerkinElmer Life Sciences) and exposed to film for 10 days.

Purification of Recombinant ADAMTSL1/Punctin-1—Of several stably transfected HEK-293F clones that were isolated, the clone with the highest production level was selected for protein purification. Cells were grown in serum-free medium (SFM II, Invitrogen) supplemented with L-glutamine in tripletier flasks (Nunc, Rochester, NY), and the medium was pooled for subsequent purification. Punctin-1 was purified from serum-free conditioned medium by affinity chromatography on nickel-Sepharose (ProBond resin, Invitrogen), utilizing the C-terminal His₆ tag, essentially as described previously (4). Protein purity was assessed by silver staining under reducing and non-reducing conditions.

Analysis of Tryptic Peptides by Ion Trap Mass Spectrometry—Tryptic peptides were generated from 1 µg of reduced and alkylated punctin-1, and the resulting tryptic peptides were analyzed by LC-MS/MS using an Agilent XCT ion trap mass spectrometer as described (41). Briefly, the peptides were separated on a Zorbax 300SB-C8 column (3.5-µm beads, 150 x 0.3 mm, Agilent) with the following gradient: 0–5 min, 5% buffer B; 5–85 min, 5–35% buffer B; 85–105 min, 35–95% buffer B; 105–115 min, 95% buffer B (where buffer A = 0.1% formic acid, and buffer B = 95% acetonitrile in 0.1% formic acid). The effluent from the column was sprayed directly into the ion trap mass spectrometer under the conditions described in Ref. 41. The scanning range was 400–2200 m/z, and collision-induced dissociation (CID) fragmentation (MS/MS) was performed on the two most intense ions in each MS spectrum, with exclusion after two spectra. Peptides modified with O-fucose glycans were identified by searching the data set for CID spectra that exhibit the characteristic neutral loss of the fucose-glucose disaccharide (dHex-Hex). The loss of this species is recognized as a 308-Da loss from the peptide molecular ion, taking into account the charge state of the respective ions in the CID spectrum. For instance, with doubly charged peptide ions, this loss produces a doubly charged fragment ion with an m/z difference of 154. Similarly, with triply charged peptide ions, this loss produces a triply charged fragment ion with an m/z difference of 102.7. Sequential loss of the glucose (Hex) followed by the fucose (dHex) gives a characteristic fragmentation pattern, permitting facile identification of modified peptides, where the most abundant fragment ion in the CID spectrum is the unglycosylated peptide (see Fig. 2) (41). This feature allows one to deduce the molecular weight of the unmodified peptide from the CID spectrum and determine which peptide is modified based on the known amino acid sequence of the protein and the specificity of the trypsin protease. The masses of the unmodified peptides, determined in the CID spectra shown in Fig. 2 and in the supplemental Data (and summarized in Table 1), were matched to the masses of the predicted tryptic peptides from human punctin-1 that contain a predicted O-fucose modification site (Cys¹-Xaa-Xaa-(Ser/Thr)-Cys²-Xaa-Xaa-Gly). Since each of these peptides has a unique mass (see Table 1), there were no ambiguities in assigning the spectra. The presence of b- and/or y-ions in the MS/MS data from fragmentation of the unglycosylated peptide confirmed the assignments. MS/MS/MS analysis of the unglycosylated peptides offered further confirmation of each peptide (data not shown). Due to the lability of the glycosidic linkage, assignment of the modified serine or threonine could not be reliably done. Thus, the assignment of the modified residue was based on the consensus sequence. Once glycopeptides were identified, additional searches were performed for unmodified peptides or for glycopeptides modified with fucose only.

	RESULTS

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

O-Linked Fucose Is Present in the Thrombospondin Type 1 Repeats of Punctin-1—Tryptic peptides from punctin-1 were analyzed by LC-MS/MS to determine whether the O-fucose consensus sequences within the TSRs were modified with O-fucose. Fragmentation of peptides modified with O-fucose glycans results in loss of the sugars, and the major product ion is the unglycosylated peptide (41). Thus, O-fucose modified peptides can be identified by searching MS/MS data for ions losing masses corresponding to the O-fucose glycan from multiply charged forms of peptide ions. Fig. 2A shows analysis of a tryptic peptide from TSR2 of human punctin-1 using this method. The top panel shows an MS spectrum of the effluent from the reversed-phase capillary high pressure liquid chromatography column at 65.7 min. The two major molecular ions correspond to triply ([M+3H]³⁺) and quadruply ([M+4H]⁴⁺) charged forms of a predicted tryptic peptide from TSR2 modified with the fucose-glucose disaccharide. The ion at m/z 1219.6 was selected for CID fragmentation, and the bottom panel shows the resulting MS/MS spectrum (Fig. 2A, bottom). The two major molecular ions correspond to sequential losses of the glucose ([M+3H-Hex]³⁺, m/z 1165.3) and the fucose ([M+3H-Hex-dHex]³⁺, m/z 1116.9) from the parent ion ([M+3H]³⁺). The molecular ion at m/z 1116.9 matches the predicted mass of the triply charged form of a tryptic peptide containing an O-fucose consensus sequence from TSR2 of human punctin-1 (Table 1). Additional confirmation of the assignment comes from the identification of several b- and/or y-fragment ions from the unglycosylated peptide in the MS/MS spectrum (Fig. 2A, bottom). In a separate experiment, the m/z 1116.9 was selected for MS³ fragmentation, which provided further confirmation of the assignment (not shown). Peptides modified with the fucose-glucose disaccharide from TSR3 (supplemental Fig. S1) and TSR4 (supplemental Fig. S3) were also identified using this approach. Additional searches revealed that the peptides from TSR3 (supplemental Fig. S2) and TSR4 (supplemental Fig. S4) also exist in the monosaccharide form. These data are summarized in Table 1. A molecular ion potentially matching a predicted peptide from TSR1 bearing the fucose-glucose disaccharide was also identified (not shown). Interestingly, this ion was 162 Da larger than predicted, suggesting the presence of an additional hexose. The peptide contains the consensus sequence for the addition of C-mannose (Trp-Xaa-Xaa-Trp) (16), providing a potential explanation for the additional 162 Da. Nonetheless, fragmentation data for this ion were ambiguous and did not conclusively support this assignment. Thus, further work must be done to determine whether the consensus sequence within TSR1 is modified (see below). The data for peptides from TSR2, TSR3, and TSR4 suggests that they are all modified with the O-fucose disaccharide. None of the peptides were found unmodified, suggesting that the glycosylation machinery is very efficient, even upon forced overexpression of punctin-1.

View larger version (26K): [in this window] [in a new window]   FIGURE 2. TSRs from punctin-1 are modified with O-fucose saccharides. A, tryptic peptides from punctin-1 were analyzed by LC-MS/MS as described under "Experimental Procedures." Searches of the MS/MS data for neutral loss of 102.7 (loss of the fucose-glucose disaccharide from a triply charged ion) revealed the spectra shown. Top panel, an MS spectrum of the column effluent at 65.7 min. M corresponds to the mass for the peptide plus dHex and Hex (sequence shown above the spectra). The two major molecular ions in the MS spectrum correspond to multiply charged forms of M ([M+4H]4+, [M+3H]3+). The other ions present in the MS spectrum represent other peptides eluting from the LC column at the same time. Bottom panel, CID fragmentation spectrum (MS/MS) of the m/z 1219.6 ion ([M+3H]3+) from the MS spectrum. The location of the parent ion (prior to fragmentation) is indicated with a diamond. The major product ions correspond to the sequential losses of a hexose ([M+3H-Hex]3+) and a deoxyhexose ([M+3H-Hex-dHex]3+) from the parent ion ([M+3H]3+). [M+3H-Hex-dHex]3+ corresponds to the triply charged form of a tryptic peptide from TSR2 of human punctin-1 that contains an O-fucose consensus sequence (sequence on top of spectrum, see Table 1 for predicted masses). Further confirmation of the assignment to this peptide comes from peptide fragment ions (b- and/or y-ions) that are indicated. Spectra of O-fucosylated peptides from TSR3 and TSR4 are shown in the supplemental data. B, incorporation of [3H]fucose into full-length punctin-1 (WT) and a truncated form (TSR1-CRD) containing only TSR1 and the cysteine-rich domain. UT indicates untransfected cells (a negative control). In both panels, immunoprecipitation (IP) of cell lysates from transfected or untransfected cells was done using anti-FLAG-M2 affinity matrix. In the left-hand panel, relevant molecular species were identified by Western blotting (IB) using an anti-FLAG polyclonal antibody. The identity of the 50-kDa species seen in the cell lysates of TSR1-CRD-expressing cells is not clear, but it may be a dimer of this truncated protein or a nonspecific reactive band since a similar reactivity is present in all lanes. The right-hand panel shows a fluorogram corresponding to the Western blot on the left. Specific incorporation of [3H]fucose is seen in wild-type punctin-1 and the TSR1-CRD construct as indicated.

View larger version (47K): [in this window] [in a new window]   FIGURE 3. Regulation of punctin-1 secretion by O-fucosylation. A, Western blotting of conditioned medium (top) from transfected HEK293F cells or cell lysate (bottom) using anti-Myc (for punctin-1), horseradish peroxidase-conjugated anti-human IgG, and anti-GAPDH. The molecular species encoding punctin-1 and secreted IgG (as a control for transfection and secretion efficiency) are indicated in the top panel. The lower panel includes a Western blot for GAPDH as an indicator of equivalent loading of protein samples. Transfections were done in triplicate using wild-type punctin-1 or the indicated mutants. B, signal intensity of secreted punctin-1 (relative to IgG) was measured as described under "Experimental Procedures," and levels of secreted protein obtained following transfection of the various punctin-1 mutants were compared with the levels of wild-type (WT) punctin. The bar graphs show the mean and S.D. for n = 3. Statistically significant differences (p = 0.005 in conditioned medium and p = 0.006 in cell lysate) between the levels of T312A+ S391A+ T451A-substituted punctin-1 and wild-type punctin-1 are indicated by the asterisk. C, Western blotting of conditioned medium (left-hand panel) from transfected COS-1 cells or cell lysate (right-hand panel) using anti-Myc (for punctin-1), anti-human IgG, and anti-GAPDH as indicated. D, quantitative comparison of protein levels in the medium or cell lysate of COS-1 cells (using data from C) normalized either to IgG (medium) or to GAPDH (cell lysate). Transfections in C and D were done in triplicate using wild-type punctin-1 or the indicated mutant. The level of statistical significance is indicated in each bar graph.

An alternative explanation for decreased secretion of triple mutant punctin-1 is that it may result from compromised folding and stability of the mutant polypeptide. Thus, as an alternative and complementary approach, we further evaluated the role of O-fucosylation by expression of wild-type punctin-1 and N251Q-substituted punctin-1 in Lec13 cells. Expression in Lec1 cells as shown above suggested that the addition of fucose to N-linked oligosaccharide was also essential for secretion since Lec1 cells are unable modify N-glycans with fucose (37). Lec13 cells are therefore expected to solely report the effects of lack of O-fucosylation in the TSRs upon expression of N251Q-substituted punctin-1. In six independent experiments in which we expressed punctin-1 and N251Q-substituted punctin-1 in fucose-starved Lec13 cells, it was either undetectable on Western analysis of 20 µl of unconcentrated conditioned medium or greatly diminished (Fig. 4, A and B). This volume typically provided robust signal in other transfected cells (e.g. Figs. 1C and 3, A and C). In contrast, Lec13 cells supplemented with 1 mM L-fucose regained robust secretion of both wild-type and N251Q-substituted punctin-1 (Fig. 4, A and B), although the levels of the latter were consistently less than the wild type, suggesting a cumulative effect of lacking O-fucosylation and N-glycosylation (Fig. 1, C and D). The data thus demonstrate that the effect of expressing punctin-1 in L-fucose-deprived Lec13 cells is similar to the effect of mutating TSR2, TSR3 and TSR4. Taken together with the mutagenesis data reported in Fig. 3, this strongly suggests that O-fucosylation is essential for optimal secretion of punctin-1.

View larger version (18K): [in this window] [in a new window]   FIGURE 4. Reduced punctin secretion in Lec13 cells. A, punctin-1 or N251Q-substituted punctin-1 (NQ) was expressed in Lec13 cells cultured with (+) or without (–)1mM L-fucose, and Western blotting of conditioned medium was done using anti-Myc. This figure shows the highest expression (of six independent experiments) obtained in the absence of fucose. WT, wild type. B, bar graph showing the mean and standard deviation (six independent transfections) of the level of punctin-1 in conditioned medium. The constructs used and whether cells were grown in the presence or absence of L-fucose are indicated below the graph. The level of statistical significance is shown.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

Here, we have extended these key observations to examine O-fucosylation in members of the largest potential group of substrates for POFUT2, and importantly, to determine the functional significance of this modification in punctin-1. We previously characterized recombinant punctin-1 from High-Five insect cells and showed that it was a glycoprotein with an affinity for extracellular matrix. Because insect cells glycosylate proteins differently from mammalian cells, we repurified punctin-1 from a stably transfected human cell line, HEK293F, that is commonly used for production of recombinant proteins. Mass spectral analysis demonstrated O-fucosylation of TSR2, TSR3, and TSR4. Interestingly, these TSRs did not have identical glycosylation since they were found to bear either a fucose monosaccharide (TSR3, TSR4) or a fucose-glucose disaccharide (TSR2, TSR3, TSR4). This differential glycosylation of TSRs may be due to the specificity of the 3-glucosyltransferase. Fringe shows a similar specificity for modifying O-fucose on some EGF repeats but not others (42, 43).

Although an O-fucosylated peptide potentially from TSR1 was also identified in the mass spectral analysis, its identity could not be confirmed. However, metabolic labeling of the TSR1-CRD construct strongly suggested that TSR1 is also modified by O-fucosylation. Although mutation of a single O-fucosylation site in punctin-1 had modest effects, mutation of the sites in all three C-terminal TSRs dramatically diminished the levels of secreted protein, along with significant accumulation of punctin-1 intracellularly.

Further validation of an essential role for O-fucosylation was obtained using Lec13 cells. However, the use of these cells in our analysis first necessitated an evaluation of the role of N-linked glycosylation in punctin-1 since during protein biosynthesis, fucose is also commonly incorporated into complex or hybrid-type N-linked oligosaccharides, and more rarely, into mucin-type O-linked oligosaccharides (44). Most ADAMTS proteases and ADAMTS-like proteins (with the exception of ADAMTS4) contain at least one N-linked oligosaccharide. The N251Q substitution in punctin-1 prevents the co-translational attachment of the N-linked core oligosaccharide, which is probably essential for optimal folding and secretion of the Protein. Subsequent to attachment of the core oligosaccharide in the endoplasmic reticulum, a further modification of the N-linked oligosaccharide by GlcNAc-TI in the Golgi apparatus is an essential prerequisite for the subsequent incorporation of fucose into complex or hybrid-type N-linked oligosaccharides (44). The level of punctin-1 in the medium of GlcNAc-TI-deficient Lec1 cells was decreased, further demonstrating that the N-linked oligosaccharide was essential for optimal secretion. Nevertheless, Lec13 cells, which are unable to incorporate fucose into any modification, would primarily report the effects of lack of incorporation of O-fucose into TSRs using N251Q-substituted punctin-1.

Lec13 cells showed a dramatic decrease in secreted wild-type punctin-1 as well as N251Q-substituted punctin-1. Taken together with the mutagenesis data, we conclude that the lack of fucosylation in each TSR has an additive effect on restricting secretion of punctin-1. The inability to detect unfucosylated peptides from TSR2, TSR3, and TSR4 in the mass spectral analysis argues that these TSRs are constitutively modified. One consideration raised by these observations is whether there might exist one or more cellular chaperone proteins that are specifically responsive to the levels of TSR O-fucosylation and that are charged with facilitating secretion of only correctly folded, and thus, fully fucosylated proteins. Relevant to this are the observations that POFUT2 only adds fucose to properly folded TSRs (18) and is present in the endoplasmic reticulum (17, 19), a compartment known to be involved in protein folding and quality control. Interestingly, OFUT1 (POFUT1 ortholog in Drosophila melanogaster) has been reported to have chaperone activity (22), suggesting that O-fucosylation of both EGF repeats and TSRs may play an important role in protein folding and/or quality control. It will also be important to investigate the role of O-fucosylation during stresses that induce the unfolded protein response since O-fucosylation may be affected under these conditions.

From the previous studies of Hofsteenge and colleagues (16), it is evident that two TSRs containing the target Ser or Thr residue but with a positively charged residue at the Xaa² position (i.e. immediately prior to the predicted modification site) were not O-fucosylated. Interestingly, TSR1 from every member of the ADAMTS superfamily has the constant sequence Cys¹-Ser-Arg-(Ser/Thr)-Cys², where Arg precedes the predicted modification site (underlined). Our present studies suggest that TSR1 is O-fucosylated, although we have not been able to identify the modified site or residue using mass spectrometry. Since all ADAMTS proteases have one or more TSRs harboring a likely consensus sequence for fucosylation, our data suggest that in ADAMTS proteases that do undergo O-fucosylation, this modification may exert a similar secretory control as in punctin-1. In the future, it will be important to experimentally determine the presence and role of O-fucosylation in individual ADAMTS proteases to inquire whether the present observations regarding punctin-1 are applicable to the entire superfamily.

	FOOTNOTES

 
^* This work was supported by National Institutes of Health Awards AR49930 (to S. A.) and GM61126 (to R. S. H.). The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

The on-line version of this article (available at http://www.jbc.org) contains four supplemental figures.

This article was selected as a Paper of the Week.

¹ To whom correspondence should be addressed: Biomedical Engineering (ND20), Cleveland Clinic Foundation, 9500 Euclid Ave., Cleveland, OH 44195. Tel.: 216-445-3278; Fax: 216-444-9198; E-mail: aptes{at}ccf.org.

² The abbreviations used are: TSR, type-1 repeats; POFUT1, protein-O-fucosyltransferase 1; POFUT2, protein-O-fucosyltransferase 2; CRD, cysteine-rich domain; CHO, Chinese hamster ovary; GAPDH, glyceraldehyde-3-phosphate dehydrogenase; MS/MS, tandem mass spectrometry; LC-MS/MS, laser chromatography-tandem mass spectrometry; CID, collision-induced dissociation; Hex, hexose; dHex, deoxyhexose; EGF, epidermal growth factor; GlcNAc-TI, N-acetylglucosaminyltransferase I.

	REFERENCES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 

1. Apte, S. S. (2004) Int. J. Biochem. Cell Biol. 36, 981–985[CrossRef][Medline] [Order article via Infotrieve]
2. Porter, S., Clark, I. M., Kevorkian, L., and Edwards, D. R. (2005) Biochem. J. 386, 15–27[CrossRef][Medline] [Order article via Infotrieve]
3. Lawler, J., and Hynes, R. O. (1986) J. Cell Biol. 103, 1635–1648[Abstract/Free Full Text]
4. Hirohata, S., Wang, L. W., Miyagi, M., Yan, L., Seldin, M. F., Keene, D. R., Crabb, J. W., and Apte, S. S. (2002) J. Biol. Chem. 277, 12182–12189[Abstract/Free Full Text]
5. Hall, N. G., Klenotic, P., Anand-Apte, B., and Apte, S. S. (2003) Matrix Biol. 22, 501–510[CrossRef][Medline] [Order article via Infotrieve]
6. Huxley-Jones, J., Apte, S. S., Robertson, D. L., and Boot-Handford, R. P. (2005) Int. J. Biochem. Cell Biol. 37, 1838–1845[CrossRef][Medline] [Order article via Infotrieve]
7. Kramerova, I. A., Kawaguchi, N., Fessler, L. I., Nelson, R. E., Chen, Y., Kramerov, A. A., Kusche-Gullberg, M., Kramer, J. M., Ackley, B. D., Sieron, A. L., Prockop, D. J., and Fessler, J. H. (2000) Development (Camb.) 127, 5475–5485[Abstract]
8. Nardi, J. B., Gao, C., and Kanost, M. R. (2001) J. Insect Physiol. 47, 997–1006[CrossRef][Medline] [Order article via Infotrieve]
9. Harris, R. J., and Spellman, M. W. (1993) Glycobiology 3, 219–224[Abstract/Free Full Text]
10. Haltiwanger, R. S., and Lowe, J. B. (2004) Annu. Rev. Biochem. 73, 491–537[CrossRef][Medline] [Order article via Infotrieve]
11. Haines, N., and Irvine, K. D. (2003) Nat. Rev. Mol. Cell. Biol. 4, 786–797[Medline] [Order article via Infotrieve]
12. Wang, Y., Shao, L., Shi, S., Harris, R. J., Spellman, M. W., Stanley, P., and Haltiwanger, R. S. (2001) J. Biol. Chem. 276, 40338–40345[Abstract/Free Full Text]
13. Moloney, D. J., Panin, V. M., Johnston, S. H., Chen, J., Shao, L., Wilson, R., Wang, Y., Stanley, P., Irvine, K. D., Haltiwanger, R. S., and Vogt, T. F. (2000) Nature 406, 369–375[CrossRef][Medline] [Order article via Infotrieve]
14. Bruckner, K., Perez, L., Clausen, H., and Cohen, S. (2000) Nature 406, 411–415[CrossRef][Medline] [Order article via Infotrieve]
15. Hofsteenge, J., Huwiler, K. G., Macek, B., Hess, D., Lawler, J., Mosher, D. F., and Peter-Katalinic, J. (2001) J. Biol. Chem. 276, 6485–6498[Abstract/Free Full Text]
16. Gonzalez de Peredo, A., Klein, D., Macek, B., Hess, D., Peter-Katalinic, J., and Hofsteenge, J. (2002) Mol. Cell. Proteomics 1, 11–18[Abstract/Free Full Text]
17. Luo, Y., Koles, K., Vorndam, W., Haltiwanger, R. S., and Panin, V. M. (2006) J. Biol. Chem. 281, 9393–9399[Abstract/Free Full Text]
18. Luo, Y., Nita-Lazar, A., and Haltiwanger, R. S. (2006) J. Biol. Chem. 281, 9385–9392[Abstract/Free Full Text]
19. Kozma, K., Keusch, J. J., Hegemann, B., Luther, K. B., Klein, D., Hess, D., Haltiwanger, R. S., and Hofsteenge, J. (2006) J. Biol. Chem. 281, 36742–36751[Abstract/Free Full Text]
20. Sato, T., Sato, M., Kiyohara, K., Sogabe, M., Shikanai, T., Kikuchi, N., Togayachi, A., Ishida, H., Ito, H., Kameyama, A., Gotoh, M., and Narimatsu, H. (2006) Glycobiology 16, 1194–1206[Abstract/Free Full Text]
21. Xu, A., Lei, L., and Irvine, K. D. (2005) J. Biol. Chem. 280, 30158–30165[Abstract/Free Full Text]
22. Okajima, T., Xu, A., Lei, L., and Irvine, K. D. (2005) Science 307, 1599–1603[Abstract/Free Full Text]
23. Rampal, R., Arboleda-Velasquez, J. F., Nita-Lazar, A., Kosik, K. S., and Haltiwanger, R. S. (2005) J. Biol. Chem. 280, 32133–32140[Abstract/Free Full Text]
24. Luo, Y., and Haltiwanger, R. S. (2005) J. Biol. Chem. 280, 11289–11294[Abstract/Free Full Text]
25. Colige, A., Sieron, A. L., Li, S. W., Schwarze, U., Petty, E., Wertelecki, W., Wilcox, W., Krakow, D., Cohn, D. H., Reardon, W., Byers, P. H., Lapiere, C. M., Prockop, D. J., and Nusgens, B. V. (1999) Am. J. Hum. Genet. 65, 308–317[CrossRef][Medline] [Order article via Infotrieve]
26. Tortorella, M. D., Burn, T. C., Pratta, M. A., Abbaszade, I., Hollis, J. M., Liu, R., Rosenfeld, S. A., Copeland, R. A., Decicco, C. P., Wynn, R., Rockwell, A., Yang, F., Duke, J. L., Solomon, K., George, H., Bruckner, R., Nagase, H., Itoh, Y., Ellis, D. M., Ross, H., Wiswall, B. H., Murphy, K., Hillman, M. C., Jr., Hollis, G. F., and Arner, E. C. (1999) Science 284, 1664–1666[Abstract/Free Full Text]
27. Stanton, H., Rogerson, F. M., East, C. J., Golub, S. B., Lawlor, K. E., Meeker, C. T., Little, C. B., Last, K., Farmer, P. J., Campbell, I. K., Fourie, A. M., and Fosang, A. J. (2005) Nature 434, 648–652[CrossRef][Medline] [Order article via Infotrieve]
28. Glasson, S. S., Askew, R., Sheppard, B., Carito, B., Blanchet, T., Ma, H. L., Flannery, C. R., Peluso, D., Kanki, K., Yang, Z., Majumdar, M. K., and Morris, E. A. (2005) Nature 434, 644–648[CrossRef][Medline] [Order article via Infotrieve]
29. Dagoneau, N., Benoist-Lasselin, C., Huber, C., Faivre, L., Megarbane, A., Alswaid, A., Dollfus, H., Alembik, Y., Munnich, A., Legeai-Mallet, L., and Cormier-Daire, V. (2004) Am. J. Hum. Genet. 75, 801–806[CrossRef][Medline] [Order article via Infotrieve]
30. Levy, G. G., Nichols, W. C., Lian, E. C., Foroud, T., McClintick, J. N., McGee, B. M., Yang, A. Y., Siemieniak, D. R., Stark, K. R., Gruppo, R., Sarode, R., Shurin, S. B., Chandrasekaran, V., Stabler, S. P., Sabio, H., Bouhassira, E. E., Upshaw, J. D., Jr., Ginsburg, D., and Tsai, H. M. (2001) Nature 413, 488–494[CrossRef][Medline] [Order article via Infotrieve]
31. Shindo, T., Kurihara, H., Kuno, K., Yokoyama, H., Wada, T., Kurihara, Y., Imai, T., Wang, Y., Ogata, M., Nishimatsu, H., Moriyama, N., Oh-hashi, Y., Morita, H., Ishikawa, T., Nagai, R., Yazaki, Y., and Matsushima, K. (2000) J. Clin. Investig. 105, 1345–1352[Medline] [Order article via Infotrieve]
32. Rao, C., Foernzler, D., Loftus, S. K., Liu, S., McPherson, J. D., Jungers, K. A., Apte, S. S., Pavan, W. J., and Beier, D. R. (2003) Development (Camb.) 130, 4665–4672[Abstract/Free Full Text]
33. Lee, N. V., Sato, M., Annis, D. S., Loo, J. A., Wu, L., Mosher, D. F., and Iruela-Arispe, M. L. (2006) EMBO J. 25, 5270–5283[CrossRef][Medline] [Order article via Infotrieve]
34. Ripka, J., Adamany, A., and Stanley, P. (1986) Arch. Biochem. Biophys. 249, 533–545[CrossRef][Medline] [Order article via Infotrieve]
35. Kumar, R., and Stanley, P. (1989) Mol. Cell. Biol. 9, 5713–5717[Abstract/Free Full Text]
36. Stanley, P. (1985) Mol. Cell. Biol. 5, 923–929[Abstract/Free Full Text]
37. Moloney, D. J., Lin, A. I., and Haltiwanger, R. S. (1997) J. Biol. Chem. 272, 19046–19050[Abstract/Free Full Text]
38. Hsieh, J. C., Kodjabachian, L., Rebbert, M. L., Rattner, A., Smallwood, P. M., Samos, C. H., Nusse, R., Dawid, I. B., and Nathans, J. (1999) Nature 398, 431–436[CrossRef][Medline] [Order article via Infotrieve]
39. Somerville, R. P., Longpre, J. M., Jungers, K. A., Engle, J. M., Ross, M., Evanko, S., Wight, T. N., Leduc, R., and Apte, S. S. (2003) J. Biol. Chem. 278, 9503–9513[Abstract/Free Full Text]
40. Nita-Lazar, A., and Haltiwanger, R. S. (2006) Methods Mol. Biol. 347, 57–68[Medline] [Order article via Infotrieve]
41. Nita-Lazar, A., and Haltiwanger, R. S. (2006) Methods Enzymol. 417, 93–111[Medline] [Order article via Infotrieve]
42. Rampal, R., Li, A. S., Moloney, D. J., Georgiou, S. A., Luther, K. B., Nita-Lazar, A., and Haltiwanger, R. S. (2005) J. Biol. Chem. 280, 42454–42463[Abstract/Free Full Text]
43. Shao, L., Moloney, D. J., and Haltiwanger, R. (2003) J. Biol. Chem. 278, 7775–7782[Abstract/Free Full Text]
44. Varki, A., Cummings, R., Esko, J., Freeze, H., Hart, G., and Marth, J. (1999) Essentials of Glycobiology, Cold Spring Harbor Laboratory Press, Cold Spring Harbor, NY

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