1 University of Cambridge, Department of Oncology, Cambridge Institute of Medical Research, Hills Road, Cambridge, CB2 2XY, UK
2 Center for Experimental Therapeutics, University of Pennsylvania School of Medicine, 421 Curie Blvd, Philadelphia, PA 19104, USA
3 National Jewish Medical and Research Center, Department of Pediatrics, 1400 Jackson Street, Colorado 80206, USA
* Author for correspondence (e-mail: sms45{at}cam.ac.uk)
Accepted 2 March 2005
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Summary |
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Key words: ERK, MAP kinase, TACE phosphorylation, TACE trafficking
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Introduction |
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To date, at least 34 ADAM genes have been described encoding mainly type 1 transmembrane proteins, most of which contain a pro-domain, a metalloprotease domain, a disintegrin and cysteine-rich domain, a transmembrane domain and an intracellular domain (ICD) (Seals and Courtneidge, 2003). Upon the synthesis of ADAMs proteins, the pro-domain inhibits the catalytic activity of the metalloprotease domain, hence its enzymatic removal in a late Golgi compartment that is a critical prerequisite for the maturation of the ADAM protein as it progresses through the secretory pathway (Borroto et al., 2003
; Schlondorff et al., 2000
). In the case of ADAM17, pro-domain cleavage occurs by pro-protein convertases and furin (Peiretti et al., 2003
; Srour et al., 2003
).
The ICD of the ADAMs proteins has been shown to be variable in length and sequence. Despite this, the most common motif present in this domain is the PxxP binding site motif for proteins containing an SH-3 domain. This has been extensively characterised for PI-3 kinase and src tyrosine kinase binding in the instances of ADAMs 12 and 15, respectively (Kang et al., 2000; Poghosyan et al., 2002
). These observations are functionally consistent with the notion that the ICD may be responsible for mediating `inside-out' regulation of metalloprotease activity or the `outside-in' regulation of cell signalling.
TACE/ADAM17 was originally identified by its ability to cleave transmembrane TNF- to soluble TNF-
in THP-1 cells (Black et al., 1997
; Moss et al., 1997
). Subsequently, many transmembrane proteins have been identified as substrates for this enzyme, e.g. TNF-Receptor 2 (Reddy et al., 2000
), IL-Receptor II (Reddy et al., 2000
; Solomon et al., 1999
), L-selectin and L1 (Borland et al., 1999
), TGF-
(Arribas et al., 1997
), erbB4/HER4 (Rio et al., 2000
), fractalkine (Garton et al., 2001
) and ß-amyloid precursor protein (Slack et al., 2001
).
Although stimulation with PMA and growth factors has been shown in most cases to enhance the shedding of transmembrane proteins, the underlying mechanisms for this tightly regulated event remain unclear. In the case of ADAM9, PKC- has been shown to be directly associated with the ICD and to be required for the shedding of HB-EGF, either after PKC-
activation or after the phosphorylation of ADAM9 by PKC-
(Izumi et al., 1998
). Similarly, the ICD of TACE has also received considerable attention as a key component in the inducible regulation of TACE activity. To date, the precise role of the ICD in TACE protein maturation and degradation remains unclear. Although the ICD may be dispensable for PMA-induced shedding (Doedens and Black, 2000
; Doedens et al., 2003
), as yet no evidence has been presented to address whether altered rates of TACE protein maturation and degradation are exhibited by these deletion constructs. As our study was in progress, phosphorylation of pro-TACE at Thr735 and Ser819 was demonstrated upon PMA and growth factor-mediated stimulation of cells. Here, extracellular signal-regulated kinase (ERK) had been shown to interact with TACE and phosphorylate TACE at Thr735 whereas the kinase responsible for the phosphorylation of Ser819 has yet to be identified. Moreover, phosphorylation of Thr735 by ERK was shown to be intrinsically required for the efficient shedding of TrkA by TACE, whereas the precise role of Ser819 phosphorylation on TGF-
shedding still remains to be defined (Diaz-Rodriguez et al., 2002
; Fan et al., 2003
).
Although ERK modification of TACE ICD has been shown to be critical in efficient inducible shedding of TrkA, the precise physiological significance of this event remains unclear. In this study, we assessed the role of ERK activation and the concurrent modification of TACE at Thr735 by analysing TACE protein maturation and trafficking from the endoplasmic reticulum (ER) to the cell surface. Our observations suggest that the activation of ERK and the consequential modification of TACE at Thr735 is a key step in the physiological regulation of inducible TACE maturation and trafficking to the cell surface.
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Materials and Methods |
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Plasmids
Full-length wild-type mouse TACE (pWT.TACE) was PCR generated from pMOS/TACE using VentTM polymerase (New England Biolabs, UK) and cloned into pcDNA3.1+/Zeo (Invitrogen). The DNA sequence of the TACE coding sequence was determined using Big Dye DNA sequencing termination mix (version 2.1, Applied Biosystems). pT735A.TACE and pT735E.TACE mammalian expression plasmids were constructed by PCR using mutated overlapping primers. The resulting cDNA fragments were cloned into pcDNA3.1+/Zeo and their nucleotide sequence verified by sequencing. TACE cDNA fragments were sub-cloned into pEGFP-N1 (BD Clontech), giving plasmids pWT.TACE-eGFP, pT735A.TACE-eGFP and pT735E.TACE-eGFP.
For carboxyl HA epitope tagging of mammalian expression constructs, TACE-derived constructs were cloned into pcDNA3.1+/HA giving the carboxyl HA-tagged TACE constructs pWT.TACE-HA, pT735A.TACE-HA and pT735E.TACE-HA. Mammalian expression plasmids for constitutively active mutated MEK-1 (pMEK-1-HA) and wild-type mouse ERK2 (pWT.ERK2-HA) were PCR cloned using the template plasmid pCAMEK/ERK2-14 (a bi-cistronic plasmid encoding constitutively active Xenopus MEK-1 and mouse ERK2). Coding sequences were fused to the HA tag by cloning into pcDNA3.1+/HA. HeLa cells stably expressing WT.TACE were generated by transfecting 103 cells using 1 µg of pWT.TACE. 48 hours after transfection the medium was removed and replaced with complete Dulbecco's medium containing 500 µg/ml Zeocin (Invitrogen). Media was replaced every 2 days for 10 days and colonies picked and expanded, before being lysed using NP-40LB and analysed by Western blotting with an anti-TACE ICD antibody (C-15).
Immunoprecipitation
Cells were washed in ice-cold PBS and lysed in 1 ml NP-40LB (50 mM Tris-HCl pH 8.0, 150 mM NaCl, 5 mM EDTA, 1% v/v NP-40, 1 mM phenylmethylsulphonyl fluoride, 20 µg/ml leupeptin, 10 µg/ml aprotinin, 1 mM NaF and 1 mM Na3VO4, 10 mM 1,10-phenanthroline, 1 µM BB-94) and the extract cleared by centrifugation at 4°C for 10 minutes at 16,110 g. 5% by volume was removed at this stage for protein analysis by western blotting. Lysates were incubated with 3 µg immunoprecipitating antibody for 3 hours with rotation at 4°C. 50 µl protein A/G-PLUS agarose (Santa Cruz Biotechnology) were added and the reactions incubated overnight at 4°C with rotation. Subsequently, the immune complexes were harvested by centrifugation at 200 g for 1 minute and then resuspended in NP-40WASH buffer (NP-40LB containing 0.1% v/v NP-40) or NP-40LB for six cycles. Immune complexes were boiled in reducing 1x Laemmli buffer and analysed by western blotting.
Transfection of mammalian cells
Cells were seeded 1 day prior to transfection, at 1.5x105 cells per 35 mm dish and at 1x104 cells on 13 mm glass coverslips (Agar Scientific, UK). DNA/FuGene 6 complexes were made in serum-free DMEM medium as recommended by the manufacturer (Roche Diagnostics, UK). Transfection mixes were incubated with cells at 37°C for 24 hours.
Radiolabelling total cell proteins
The medium was removed from transfected cells and replaced with phosphate-free DMEM (Invitrogen) containing the above supplements and 2 mCi [33P]orthophosphate for 6 hours (Amersham Pharmacia). Cells were washed twice with ice-cold PBS, lysed in cold NP-40LB and lysates cleared by centrifugation. TACE was immunoprecipitated overnight and immune complexes were washed six times using ice-cold NP-40WASH before being resolved by SDS-PAGE, transferred to nitrocellulose membrane and autoradiographed.
Laser-scanning confocal microscopy
Transfected HeLa cells were fixed in 20°C methanol for 5 minutes then washed three times in PBS. Coverslips were incubated in primary antibody for 1 hour followed by three washes in PBS or as recommended by the manufacturer. Texas Red (1:200, Stratech Scientific, UK) or Alexa 488/546 donkey anti-goat antibody (Molecular Probes, USA) secondary antibodies were used. Coverslips were incubated in secondary antibody for 1 hour before being washed three times in PBS and mounted in Vectashield mounting medium containing DAPI or medium alone (Vectashield Laboratories, UK). Transfected cells were visualised using a Zeiss LSM5 microscope, using 100x objectives. The z-stack images were analysed using Zeiss LSM Image browser software and Adobe Photoshop 7 and a selected single z-slice is presented in each case.
Pulse-chase analysis of TACE
COS-7 cells were seeded at 2x106 cells per 10 cm dish and incubated overnight. The following day cells were transfected using 2 µg pWT.TACE, pT735A.TACE and 6 µg pT735E.TACE using FuGene 6 reagent. 6 hours into the incubation, all cells were treated with 50 µM leupeptin and the incubation continued for 18 hours. The transfected cells were starved for 1 hour in cysteine- and methionine-deficient DMEM medium (containing 50 µM leupeptin) and 210 µCi Redivue 35S PRO-MIX 35S-Cys/35S-Met in vitro cell labelling mix (Amersham Biosciences) was added and the incubation continued for 3 hours at 37°C. The cells were washed twice with ice-cold PBS and then chased in complete DMEM medium (lacking leupeptin) and cell lysates prepared as outlined by (Schlondorff et al., 2000). All lysates were pre-cleared using 50 µl protein A/G-PLUS for 1 hour before TACE was immunoprecipitated by addition of 10 µg of anti-TACE antibody (C-15) for 3 hours before adding 50 µl protein A/G-PLUS agarose beads and the incubation continued overnight at 4°C. Immune complexes were harvested and removed from the agarose beads by heating in 1x Laemmli buffer at 95°C for 5 minutes and all glycoproteins isolated and analysed using concanavalin A sepharose as described (Schlondorff et al., 2000
).
Biotinylation of cell surface proteins
Transfected cells were incubated on ice for 5 minutes, washed and cell surface proteins biotinylated with 0.5 mg/ml Sulpho-NHS-LC-biotin [sulphosuccinimidyl-6-(biotinamido)hexanoate] as recommended by the manufacturer (Pierce). Biotinylated cells were lysed in 1.5 ml NP-40LB and TACE-HA derivatives immunoprecipitated overnight before being washed six times in ice-cold NP-40LB and resolved using 10% SDS-PAGE followed by western blotting using streptavidin-HRP conjugated antibodies as recommended by the manufacturer (Pierce). Prior to immunoprecipitation, 50 µl whole cell lysate (WCL) was removed for future protein analysis (by Western blotting) to elucidate positive expression of transiently expressed proteins.
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Results |
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Next we addressed whether TACE can co-compartmentalise and consequently be phosphorylated with activated ERK in intact cells by coexpression of TACE with constitutively active MEK-1 and WT.ERK2 (Robinson and Cobb, 1997). Therefore, we transfected COS-7 cells with pWT.TACE and pWT.ERK2 in the presence or absence of pCA.MEK-1 and incubated the cells with [33P]orthophosphate for 6 hours, as demonstrated for TNF-Receptor 1 phosphorylation (Cottin et al., 1999
). When cells were co-transfected with TACE, constitutively active MEK-1 and WT.ERK2, pro-TACE (120 kDa) was maximally phosphorylated in an ERK activation-dependent manner (Fig. 1A, top panel), which is in good agreement with previously published observations (Diaz-Rodriguez et al., 2002
). However, in light of the recent observations that TACE may also undergo phosphorylation at Ser819 upon ERK activation (Fan et al., 2003
), we next asked whether the ERK-dependent phosphorylation of pro-TACE observed (Fig. 1A) was due to phosphorylation at Thr735. Therefore, we expressed WT.TACE and T735A.TACE in COS-7 cells in the presence of CA.MEK-1 and WT.ERK2, purifying TACE by immunoprecipitation and analysing its phosphorylation status using western blotting with a phosphothreonine-specific antibody (
-pThr). A 120 kDa protein corresponding to pro-WT.TACE was phosphorylated in the presence of active ERK2, which was abolished upon mutation of Thr735 to Ala735 (T735A.TACE) (Fig. 1B, top panel). Interestingly, TACE was detected by western blotting as a very faint doublet band (highlighted by arrows), which is strongly indicative of post-translational modification of proteins by phosphorylation. Collectively, these observations suggest that ectopic pro-TACE (120 kDa) can undergo phosphorylation at Thr735 in an ERK activation-dependent manner in COS-7 cells.
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Active ERK induces WT.TACE-eGFP relocalisation
Activation of ERK and the subsequent phosphorylation of TNF-Receptor 1 and leukaemia inhibitory factor receptor, alters their subcellular compartmentalisation and is one way the activity of such proteins is tightly regulated upon their exposure to mitogenic stimuli (Blanchard et al., 2000; Cottin et al., 2001
). Thus, we asked if ER-resident TACE could be mobilised in an ERK-dependent manner by coexpressing it with constitutively active MEK-1-activated ERK in HeLa cells. Coexpression of CA.MEK-1 or WT.ERK2 with WT.TACE-eGFP and phospho-null T735A.TACE-eGFP did not affect the overall subcellular distribution of the TACE proteins (Fig. 3A). However, coexpression of constitutively active MEK-1 and WT.ERK with WT.TACE-eGFP resulted in the redistribution of WT.TACE-eGFP from the ER to intracellular vesicular structures that are distinct from the ER or are ER-derived. Similarly, upon analysis of T735A.TACE-eGFP, we found that this mutant derivative remained compartmentalised predominantly in the ER (Fig. 3B). Therefore, we concluded that in the presence of active ERK, TACE-eGFP no longer seems to be significantly localised in the ER network and that residue Thr735 is critically important for this change in TACE-eGFP distribution to occur.
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Although TACE has been demonstrated to undergo phosphorylation at Ser819 in an ERK-dependent manner, we addressed the exclusive role of Thr735 modification on pro-TACE turnover using pulse-chase analysis. Consequently, for T735E.TACE to be visualised as pro-T735E.TACE, we increased the amount of plasmid used in preparation of the transfection mix, in comparison to the amounts used for Fig. 5A. We compared the turnover rates of expressed pro-T735E.TACE with pro-WT.TACE and pro-T735A.TACE (Fig. 5C). Our findings suggested that expressed pro-WT.TACE and pro-T735A.TACE had approximate half-lives that spanned 3-6 and 6-12 hours, respectively. In contrast, expressed pro-T735E.TACE had a significantly shorter half-life that spanned 0-3 hours, after which mature T735E.TACE levels were observed to diminish.
Taken together, these observations suggest that modification of TACE at Thr735 may be responsible for the progression of pro-TACE through the secretory pathway permitting its proteolytic processing to mature TACE, or may be responsible for its degradation.
ERK-dependent phosphorylation of TACE at Thr735 signals translocation of TACE to the cell surface
Following our previous observations, we then addressed whether the cell surface levels of TACE may be regulated by ERK phosphorylation at Thr735. Accordingly, we analysed cell surface HA tagged mature TACE expression upon stimulating TACE-expressing HeLa cells with PMA. Transfected HeLa cells expressing pWT.TACE-HA were stimulated with 1 µM PMA or carrier (DMSO) over a time course of 30 minutes. Cells were surface biotinylated and total TACE immunoprecipitated using an anti-HA antibody and immune complexes analysed by western blotting with streptavidin-HRP. A 100 kDa TACE species (representative of mature TACE) was observed to maximally increase at the cell surface after 10 minutes of stimulation with PMA, after which it declined (Fig. 6A). This result is consistent with the observation that WT.TACE-eGFP localisation is modified when cells are treated with PMA. Upon analysis of the whole cell lysates using western blot analysis with an anti-HA antibody, an intracellular TACE species corresponding to 120 kDa (representative of pro-TACE) was positively detected, which transiently declined in response to stimulating cells with PMA. Interestingly, TACE species corresponding to mature TACE (100 kDa) were readily detected after purification in immune complexes (as highlighted in Fig. 5), probably owing to a relatively low abundance, as only 3% of the total lysates were analysed to determine pro-TACE expression levels.
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To address whether the PMA-mediated transient increase in cell surface TACE was due to ERK-dependent phosphorylation of pro-TACE at Thr735, the same experiment was repeated using the expression constructs for WT.TACE-HA and T735A.TACE-HA. Additionally, cells were pre-treated with the MEK-1 inhibitor U0126 (or DMSO) for a period of 30 minutes and each set of cells stimulated with PMA for 5 and 10 minutes prior to the biotinylation of cell surface proteins. After TACE was immunoprecipitated, immune complexes were resolved and western blotted against streptavidin-HRP. A 100 kDa species of cell surface TACE (corresponding to mature TACE) increased in quantity following exposure to PMA for 5 and 10 minutes, which could be abrogated upon the pre-incubation of TACE-expressing cells with U0126 (Fig. 6B). Pro-TACE expression was determined to be positive in these cells by analysis of equal volumes of whole cell lysates by western blotting using an anti-HA antibody. Moreover, partial intracellular depletion of expressed pro-TACE in response to PMA stimulation was observed (as seen in Fig. 6A).
In cells expressing T735A.TACE-HA, no biotinylated TACE species corresponding to mature TACE (100 kDa) were detected after 5 or 10 minutes of stimulation of cells with PMA or 10 minutes with carrier (Fig. 6C). Similarly, cell lysates were analysed for the expression of T735A.TACE-HA using western blotting and were found to express TACE positively as a 120 kDa species that did not show any indication of being intracellularly depleted in response to the PMA treatment of cells. Moreover, HeLa cells expressing pWT.TACE-eGFP or pT735A.TACE-eGFP at 18 hours post-transfection were stimulated with DMSO (30 minutes) or 1 µM PMA and cells were fixed at timed intervals and visualised using immunofluorescence microscopy. Upon stimulation of cells with PMA at 10, 20 and 30 minutes, a punctate staining pattern (readily distinct from the ER staining pattern seen in Fig. 2A) was observed for WT.TACE-eGFP expression and not for T735A.TACE-eGFP expression (Fig. S5 in supplementary material). Collectively, these observations suggest that HeLa cells expressing ectopic TACE exhibit increased amounts of mature TACE at the cell surface in response to PMA stimulation and that this occurs owing to TACE protein trafficking and phosphorylation at Thr735 in an active ERK-dependent manner.
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Discussion |
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In this study, we addressed how the exclusive ERK-directed modification of Thr735 in the TACE ICD affects TACE trafficking. Initially, using the pharmacological antagonist U0126 to inhibit ERK activation and immunodepletion of activated ERK (derived from stimulated THP-1 and U937 cells) followed by in vitro kinase of supernatants toward GST fused mutants of the TACE ICD, we confirmed that the TACE ICD is inducibly phosphorylated at Thr735 in vitro and is dependent upon ERK activation. In addition to precisely mapping the ERK phosphorylation site to Thr735 in TACE, we demonstrated that pro-TACE compartmentalises with active ERK and consequently undergoes phosphorylation at Thr735. Moreover, the inducible phosphorylation of pro-TACE at Thr735 was reported in intact HEK-293 cells with which our data is in very strong agreement (Diaz-Rodriguez et al., 2002). These authors found that the optimum inducible shedding of TrkA was dependent upon ERK-mediated phosphorylation at Thr735 of TACE (Diaz-Rodriguez et al., 2002
).
Consequently, we pursued the hypothesis that pro-TACE phosphorylation by ERK may be required as a signal for its subcellular translocation from the ER in HeLa cells, permitting its maturation, presumably by furin and pro-protein convertases (Borroto et al., 2003; Endres et al., 2003
; Peiretti et al., 2003
; Srour et al., 2003
). Although the consequences of stimulating cells with PMA on TACE activation has been addressed in this context, the majority of studies have only touched upon the underlying effects on TACE protein trafficking (Diaz-Rodriguez et al., 2002
; Endres et al., 2003
). Upon the transient expression of WT.TACE, we found it to reside predominantly in the ER, which we hypothesised may serve as an intracellular pool of inactive TACE that can be rapidly mobilised and proteolytically activated upon cell stimulation. These observations are in good agreement with previously published data where TACE has been shown to reside in the ER (Diaz-Rodriguez et al., 2002
; Schlondorff et al., 2000
), and further demonstrates that an inability to phosphorylate TACE does not affect its basal localisation. However, previous attempts to show an intracellular redistribution of TACE by immunofluorescence microscopy after stimulating COS-7 expressing TACE cells with PMA for 30 minutes have been inconclusive (Schlondorff et al., 2000
). We propose that this may have been due to differences in the amounts of PMA used during stimulation (we used approximately 20 times excess by comparison), as in our hands expressed TACE translocating to the cell surface from an intracellular ER store in HeLa cells occurs transiently and as rapidly as 5-10 minutes after PMA stimulation and also exhibits an intracellular staining pattern distinct to ER staining (Fig. S5 in supplementary material).
Although endogenous TACE has also been detected at the cell surface (Borroto et al., 2003; Doedens and Black, 2000
; Schlondorff et al., 2000
), the precise mechanisms and the role of ERK mediated TACE phosphorylation in this context maybe more complex than envisaged. Taken together with the observation that purified T735E.TACE can correspond to the molecular mass of mature TACE, we have two hypotheses that are currently being explored in model cell systems: (1) ERK-mediated phosphorylation of pro-TACE may cause it to translocate from the ER to the TGN, followed by translocation to the cell surface; and/or (2) ERK-mediated phosphorylation of cell-surface mature TACE (at Thr735) may signal the internalisation and lysosomal degradation of TACE.
First, in support of the role of Thr735 phosphorylation in mediating TACE translocation from the ER to the cell surface, 120 kDa pro-TACE was the predominant TACE species that underwent phosphorylation by ERK in COS cells. Our observation that T735E.TACE-eGFP co-localises significantly with the markers for ER-Golgi transport (Sec-23) and the TGN marker (TGN-46), coupled with it having the molecular mass of mature TACE, supports the hypothesis that Thr735 phosphorylation may serve to translocate TACE from the ER through the secretory pathway, in HeLa cells. Consequently, T735E.TACE-eGFP may also confer resistance to Endo-H treatment in comparison to ER-resident TACE derivatives (Schlondorff et al., 2000). Additionally, by using pulse-chase analysis we found that T735E.TACE was processed from pro-TACE to mature TACE significantly faster than WT.TACE and T735A.TACE. In our study, WT.TACE matured significantly quicker than endogenous TACE in COS-7 cells possibly because our study analysed expressed TACE (Schlondorff et al., 2000
). Additionally, these findings are also consistent with the half-lives of expressed ADAM9 and ADAM15 (Lum et al., 1998
; Roghani et al., 1999
). Moreover, increased biotinylated cell surface TACE in the presence of PMA stimulation and a partial (but obvious) decrease in intracellular pro-TACE levels further support ERK-mediated anterograde trafficking of TACE. Collectively, these observations are supported by our findings where WT.TACE-eGFP is seen to reside in an intracellular compartment distinct from the ER (or ER derived compartments) upon PMA stimulation of cells using immunofluorescence microscopy (Fig. S5 in supplementary material).
Second, based upon previous observations, a phorbol ester-inducible decrease in the surface pool of functional TACE in the cell has been demonstrated (Doedens and Black, 2000; Endres et al., 2003
). In this context, it is also conceivable that phosphorylation of TACE at Thr735 may be involved in routing cell surface TACE for lysosomal degradation. This is supported in part by our observations that T735E.TACE has the same molecular mass as mature TACE (100 kDa), can colocalise significantly with early endosomes and the lysosomal marker LAMP1 (Fig. S4 in supplementary material) and in comparison to WT.TACE and T735A.TACE, has a relatively short half-life and low abundance in cell lysates. Additionally, it has been shown that TACE catalytic activity is a prerequisite for TACE to undergo endocytosis from the cell surface (Doedens and Black, 2000
). Consequently, we propose that the 100 kDa T735E derivative of TACE may constitute a catalytically active form of TACE, based upon its molecular mass (Schlondorff et al., 2000
), and due to it positively co-localising with the endosomal marker EEA1 (Fig. S4 in supplementary material). However, further work to address these issues is warranted.
Therefore, despite the ICD of TACE being dispensable for inducible TACE shedding, its potential regulatory properties in TACE protein trafficking and activation are becoming increasingly clear. Supported by the fact that the TACE ICD can interact with key signalling components such as protein tyrosine phosphatase 1 (Zheng et al., 2002) and coupled with the fact that TACE ICD can undergo phosphorylation, a novel (and critical) role for the TACE ICD in regulating the catalytic status and the steady-state levels of intracellular TACE is becoming apparent.
In summary, we have assigned a potential role for the ERK-mediated modification of TACE ICD at Thr735. This is based on our observations that expressed pro-TACE becomes phosphorylated by ERK in intact cells and that one of the consequences of this is the inducible translocation of expressed TACE from the ER to the cell surface (which is dependent upon ERK activation), after which it may undergo internalisation and degradation. Collectively, our observations suggest a novel function for the TACE ICD in TACE protein trafficking, which is dependent upon MAPK phosphorylation.
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Acknowledgments |
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Footnotes |
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References |
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