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Molecular and Cellular Biology, November 2005, p. 9324-9339, Vol. 25, No. 21
0270-7306/05/$08.00+0     doi:10.1128/MCB.25.21.9324-9339.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Soluble Axl Is Generated by ADAM10-Dependent Cleavage and Associates with Gas6 in Mouse Serum

Vadim Budagian,^1,* Elena Bulanova,^1, Zane Orinska,¹ Erwin Duitman,¹ Katja Brandt,¹ Andreas Ludwig,² Dieter Hartmann,³ Greg Lemke,⁴ Paul Saftig,² and Silvia Bulfone-Paus¹

Department of Immunology and Cell Biology, Research Center Borstel, D-23845 Borstel,¹ Institute of Biochemistry, Christian Albrechts University, D-24118 Kiel, Germany,² Department of Human Genetics, KU Leuven, and Flanders Interuniversity Institute for Biotechnology (VIB-4), B-3000 Leuven, Belgium,³ Molecular Neurobiology Laboratory, Salk Institute for Biological Studies, San Diego, California 92186⁴

Received 15 May 2005/ Returned for modification 8 June 2005/ Accepted 13 August 2005

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

 
Axl receptor tyrosine kinase exists as a transmembrane protein and as a soluble molecule. We show that constitutive and phorbol 12-myristate 13-acetate-induced generation of soluble Axl (sAxl) involves the activity of disintegrin-like metalloproteinase 10 (ADAM10). Spontaneous and inducible Axl cleavage was inhibited by the broad-spectrum metalloproteinase inhibitor GM6001 and by hydroxamate GW280264X, which is capable of blocking ADAM10 and ADAM17. Furthermore, murine fibroblasts deficient in ADAM10 expression exhibited a significant reduction in constitutive and inducible Axl shedding, whereas reconstitution of ADAM10 restored sAxl production, suggesting that ADAM10-mediated proteolysis constitutes a major mechanism for sAxl generation in mice. Partially overlapping 14-amino-acid stretch deletions in the membrane-proximal region of Axl dramatically affected sAxl generation, indicating that these regions are involved in regulating the access of the protease to the cleavage site. Importantly, relatively high circulating levels of sAxl are present in mouse sera in a heterocomplex with Axl ligand Gas6. Conversely, two other family members, Tyro3 and Mer, were not detected in mouse sera and conditioned medium. sAxl is constitutively released by murine primary cells such as dendritic and transformed cell lines. Upon immobilization, sAxl promoted cell migration and induced the phosphorylation of Axl and phosphatidylinositol 3-kinase. Thus, ADAM10-mediated generation of sAxl might play an important role in diverse biological processes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

 
Receptor tyrosine kinases (RTKs) play fundamental roles in diverse cell functions, including proliferation, differentiation, survival, migration, and metabolism (16). Axl RTK (also known as Ark, Ufo, and Tyro7) is the prototype of a family of transmembrane receptors, which also includes Tyro3 (also known as Sky, Brt, Etk, Tif, Dtk, and Rse) and Mer (c-Eyk, Nyk, and Tyro12) (34, 44, 64). They share a distinct molecular structure characterized by two immunoglobulin-like motifs and two fibronectin type III repeats in their extracellular domain and a cytoplasmic domain that contains a conserved catalytic kinase region (34, 44). Axl, Tyro3, and Mer are variably expressed in neural, lymphoid, vascular, and reproductive tissues and in different primary cells and tumor cell lines (11, 41, 42). Mutant mice that lack these three receptors have a defective phagocytic clearance of apoptotic cells and impaired spermatogenesis (41) and develop a severe lymphoproliferative disorder accompanied by broad-spectrum autoimmunity (42).

A common heterophilic ligand for these RTK family members is Gas6, a vitamin K-dependent protein that is widely secreted by most tissues, including the lungs, intestine, and vascular endothelium (43). Gas6 is the product of growth arrest-specific gene 6, which was initially cloned from serum-starved fibroblasts and shares about 44% sequence identity and similar domain organization with protein S, a negative regulator of blood coagulation (48). Recent studies indicate that the Gas6/Axl system plays an important role in vascular biology (46). A large amount of experimental evidence supports a role for Gas6/Axl signaling in cell growth and protection from apoptosis in normal and cancer cells (10, 24, 31). Axl activation results in autophosphorylation and phosphorylation of cytoplasmic substrates, including phosphatidylinositol 3-kinase (PI3K), Akt, S6K, Src kinase, ERK, p38, STAT3, and NF-B (2, 29, 32, 35, 62, 68).

The extracellular regions of Axl, Tyro3, and Mer contain similar combinations of structural motifs, which are also observed in the receptor-type protein tyrosine phosphatases and adhesion molecules of the cadherin and immunoglobulin superfamily (67). Several studies demonstrated that Axl could mediate cell adhesion and aggregation through homotypic ectodomain associations (9, 23). Both murine and human Axl proteins undergo proteolytic processing to yield a soluble form of this molecule. Murine Axl is cleaved extracellularly to generate a soluble ectodomain of approximately 65 kDa (23), whereas cleavage of human Axl is mapped to the 14-amino-acid (aa) stretch in the extracellular region and corresponds to the soluble form with a higher molecular mass of 80 kDa (50). Soluble Axl (sAxl) is present in cell-conditioned medium of tumor cells growing in vivo and in vitro and in the sera of humans, mice, and rats (23, 50). However, the identities of the sAxl-generating protease(s) and the mechanism(s) that account for this process remain unknown.

Ectodomain shedding has emerged as an important posttranslational mechanism to regulate the functions of various integral membrane-bound proteins, including adhesion molecules, cytokines, growth factors, and their receptors (57, 60). Both membrane-bound and soluble members of the protease superfamily can mediate this process (14). Yet, metalloproteinases of the zinc-dependent ADAM family (for a disintegrin and metalloproteinase) were shown to be responsible for the cleavage of the majority of shed proteins (27, 57). The ADAMs are type I membrane-anchored glycoproteins which play important roles in fertilization, neurogenesis, and angiogenesis and mediate the shedding of various membrane-bound molecules (14, 57). Among these family members, ADAM10/Kuzbanian and ADAM17/TACE (for tumor necrosis factor alpha [TNF-]-converting enzyme) are particularly important in the context of ectodomain generation (57). They are involved in the proteolysis of various substrates, including epidermal growth factor receptor ligands (14, 55), TNF- and its receptors (12, 25), amyloid precursor protein (61), Notch (13), Notch ligand Delta (60), N-cadherin (54), fractalkine (38), and many others.

In the present study, we demonstrate that a soluble variant of murine Axl RTK is constitutively generated from the full-length transmembrane molecule through defined proteolytic cleavage and identify ADAM10 as the major metalloproteinase responsible for this process. We provide several lines of experimental evidence which support a functional role for this soluble molecule. Importantly, sAxl is constitutively present in mouse serum and cell-conditioned medium in combination with Gas6, which may affect Gas6 bioavailability and activity. Thus, our results link the proteolytic cleavage of Axl and Gas6 function, suggesting that maintenance of a dynamic equilibrium between serum levels of sAxl and Gas6 might play an important regulatory role.

	MATERIALS AND METHODS

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Cytokines, antibodies (Abs), inhibitors, and recombinant proteins. Recombinant human interleukin-15 (IL-15), granulocyte-macrophage colony-stimulating factor (GM-CSF), and TNF- were purchased from TEBU. Lipopolysaccharide (LPS) derived from Salmonella enterica serovar Friedenau was kindly provided by H. Brade (Research Center Borstel, Borstel, Germany). Phorbol 12-myristate 13-acetate (PMA) and anti-ß-actin Abs were purchased from Sigma-Aldrich. Abs against Axl (M-19), Gas6 (N-20), and PI3K (Z-8) were from Santa Cruz Biotechnology; antiphosphotyrosine Abs (RC20) were from BD Biosciences, and anti-ADAM10 Abs were from Chemicon. Recombinant murine Gas6, rat anti-mouse Gas6, biotinylated goat anti-mouse Gas6, Axl, Mer, and Tyro3 (Dtk) Abs and Axl-Fc and IL-3R-Fc chimeras were purchased from R&D Systems.

The broad-spectrum hydroxamic acid-based metalloproteinase inhibitor GM6001 and the respective negative control compound were purchased from Calbiochem. GW280264X (a potent inhibitor of TACE and ADAM10 metalloproteinases) was previously described (1, 38).

Cell culture, stimulation, and transfection conditions. Ras-Myc-retrovirus-immortalized TACE^–/– (generously provided by S. Rose-John, Christian-Albrechts-University, Kiel, Germany), simian virus large T antigen (SV-T)-immortalized ADAM10^–/–, primary Axl^–/– mouse embryo fibroblasts (MEFs), and respective wild-type (WT) cells were generated and characterized as described elsewhere (3, 36, 53). Axl^–/– MEFs were immortalized by stable transfection with the simian virus 40 large T antigen expression vector pMSSVLT (58). Murine plasmacytoma J558L (19), murine mammary adenocarcinoma TS/A (17), murine fibrosarcoma L929 (ECACC 85011425), its TNF--resistant derivative L929R, and primate fibroblast COS-7 (ATCC CRL-1651) cell lines were maintained in RPMI 1640 medium, and MEFs were cultured in Dulbecco modified Eagle medium. Culture medium was supplemented with 10% fetal calf serum (FCS), 2 mM L-glutamine, 100 U/ml penicillin, and 100 µg/ml streptomycin. Cells were stimulated with PMA (200 ng/ml) in FCS-free medium.

Bone marrow-derived dendritic cells (DCs) were generated as previously described (15). Briefly, bone marrow cells were flushed from the femurs and tibias of mice and erythrocytes were lysed. Cells were grown in RPMI 1640 medium supplemented with 10% FCS, 2 mM L-glutamine, 50 µM ß-mercaptoethanol, antibiotics, and 20 ng/ml GM-CSF. On day 3, fresh medium with 20 ng/ml GM-CSF was added and on day 6, half of the cell-free culture supernatant was replaced with fresh medium containing 10 ng/ml GM-CSF. On day 8, cells were harvested, washed twice, and incubated with LPS (10 ng/ml) for 24 h. Purity was routinely >95% as determined by fluorescence-activated cell sorter analysis.

ADAM10^–/– MEFs were reconstituted with bovine hemagglutinin-tagged ADAM10 cDNA in a retroviral expression vector based on pCXbsr (kindly provided by F. Fahrenholz, Institute of Biochemistry, Mainz, Germany) as previously described (1, 38). COS-7 cells were transfected with Lipofectamine 2000 (Gibco-Invitrogen) and analyzed 48 h posttransfection. Transfection efficiency was confirmed by Western blotting with specific Abs.

The small interfering RNA (siRNA) method was used to knock down ADAM10 expression. siRNA oligonucleotides targeting ADAM10 expression were purchased from Ambion, whereas transfection with scrambled oligonucleotides was used as a control. Cells were transfected by jetSI-FluoF siRNA transfection reagent (Eurogentec) with 50 nM siRNA. Forty-eight hours posttransfection, part of the cells was analyzed for specific depletion of ADAM10 protein by Western blotting with anti-ADAM10 Abs. Transfection efficiency was about 80 to 90% as detected by fluorescence microscopy (data not shown).

Mice. Female mice of the inbred strains BALB/c, CH3, and C57BL/6 were obtained from Charles River breeding laboratories. Axl^+/+, Axl^+/–, and Axl^–/– mice (41, 42) were bred in the Research Center Borstel under specific-pathogen-free conditions. Mice were bled from the tail vein, and sera were analyzed by enzyme-linked immunosorbent assay (ELISA).

Plasmid construction and deletion analysis. Axl (ARK) cDNA in the pRK5 vector was kindly provided by P. Bellosta (European Institute of Oncology, Milan, Italy). Three Axl deletion mutants were created by removing partially overlapping 14-aa sequences (⁴³⁸VSEPPPRAFSWPWW⁴⁵¹, ⁴⁴²RAFSWPWWYVLLGA⁴⁵⁶, and ⁴³²QPLHHLVSEPPPRA⁴⁴⁶) in the membrane-proximal region of murine Axl and designated Axl1, Axl2, and Axl3, respectively. For the generation of the deletion mutants, an inverse PCR strategy was utilized. Pairs of primers (Axl1 sense, 5'-TATGTACTGCTGGGAGCACTTGTG-3'; Axl1 antisense, 5'-CAGATGGTGGAGTGGCTGTCCTTG-3'; Axl2 sense, 5'-AGGTGGGGGTTCACTCAC-3'; Axl2 antisense, 5'-CTTGTGGCTGCCGCCTGCGTC-3'; Axl3 sense, 5'-TCCTTGCCCTGGGCGCCAGGG-3'; Axl3 antisense, 5'-TTCTCGTGGCCTTGGTGGTAT-3') in the Axl coding sequence were designed in such a way that, after PCR amplification, the complete plasmid pRK5 was obtained again, lacking only the bases located between the two primers. The PCR products obtained were subsequently phosphorylated and ligated. The identities of the deletion-containing constructs were verified by standard DNA sequencing.

ELISA. Concentrations of Axl, Gas6, and Tyro3 in cell supernatants, lysates, and mouse sera were evaluated by DuoSet ELISA kits (R&D Systems) according to the manufacturer's recommendations. Soluble Mer was detected with rat anti-mouse Mer and biotinylated goat anti-mouse Mer Abs (both from R&D Systems). In brief, a 96-well plate (Greiner) was coated and incubated overnight at 4°C with 1 µg/ml of rat anti-Mer Abs. Wells were blocked with 2% bovine serum albumin in PBS for 2 h. Samples (50 to 100 µl/well) were added to the plate, which was incubated overnight at 4°C. Serial dilutions of murine recombinant Mer were used for standardization. Bound Mer was detected with biotinylated anti-Mer Abs at a concentration of 1 µg/ml, followed by incubation with streptavidin-peroxidase. Axl/Gas6 heterocomplexes in mouse sera were detected by a two-site ELISA. Plates were coated with monoclonal anti-Axl Abs, and Axl/Gas6 heterocomplexes in samples were detected with polyclonal biotinylated goat anti-mouse Gas6 Abs, followed by incubation with streptavidin-peroxidase. A chromogenic substrate (R&D Systems) was used for visualization, and the reaction was stopped after 20 min of incubation by addition of 1 N H₂SO₄. Optical density was determined at 450 nm with an ELISA reader (Dynatech). Anti-Axl or anti-Gas6 Abs did not show cross-reactivity for Gas6 or Axl, respectively.

Immunoprecipitation and Western blotting. NP-40 (0.5% final concentration) and a cocktail of protease inhibitors were added to cell supernatants or sera, and immunoprecipitation with biotinylated anti-Axl Abs was performed for 2 h at 4°C. Immunocomplexes were captured on streptavidin-agarose (Perbio Science). To analyze glycosylation, the samples after immunoprecipitation were treated with 250 mU of N-glycosidase F (Roche) for 3 h at 37°C according to the manufacturer's instructions. Samples were resuspended in sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis (PAGE) sample buffer (62.5 mM Tris-HCl, pH 8.0, 1% glycerol, 2% SDS, 5% ß-mercaptoethanol, 0.01% bromophenol blue), boiled for 5 min, and subjected to 10% SDS-PAGE. The resolved proteins were transferred onto nitrocellulose (Bio-Rad). Blots were blocked for 1 h in PBS containing 0.05% Tween 20 and 3% bovine serum albumin (Sigma-Aldrich). After incubations with primary and secondary Abs and washing with PBS-0.05% Tween 20, visualization of specific proteins was carried out by the enhanced-chemiluminescence method with enhanced-chemiluminescence Western blotting detection reagents (Amersham Pharmacia) according to the manufacturer's instructions. Cellular extracts were prepared and analyzed by Western blotting as described elsewhere (19).

Reverse transcription (RT)-PCR. RNA was extracted from cells with TRIZOL reagent, and cDNA was synthesized from 5 µg of total RNA by using random oligonucleotides as primers and a SuperScriptII kit (all reagents were from Gibco-Invitrogen). cDNA was amplified by a standard PCR procedure as described previously (19). The following primers were used: murine Axl (473 bp) sense, 5'-CTCGGGGACCAGCCAGTGTTC-3'; murine Axl antisense, 5'-GGCCGGTCTCGAGGGTTCAGTT-3'; ß-actin (500 bp) sense, 5'-GTGGGGCGCCCCAGGCACCA-3'; ß-actin antisense, 5'-CTCCTTAATGTCACGCACGATTTC-3'. All primers were purchased from Metabion. Amplification of the ß-actin message was used to normalize the amount of cDNA used. A mock PCR (without cDNA) was included to exclude contamination in all experiments.

Flow cytometric analysis. Adherent cells were harvested from culture plates with Accutase (PAA Laboratories). Axl, Mer, or Tyro3 expression was evaluated by incubation of cells with biotinylated goat anti-mouse Axl, Mer, or Tyro3 Abs, respectively, followed by incubation with streptavidin-fluorescein isothiocyanate, and analyzed by flow cytometry with a FACScalibur (Becton Dickinson) and CellQuest software. Negative controls consisted of biotinylated, isotype-matched Abs (BD PharMingen). The fluorescence signal of the labeled cells was calculated as the median fluorescence intensity of the cell population.

Wound-healing assay. Plates were coated with 10 µg/ml of Axl-Fc or IL-3R-Fc (control) chimeric protein. Exponentially growing cells (2 x 10⁶) were plated onto coated plates in complete growth medium. After 18 h, the monolayers of cells were wounded by manual scratching with a pipette tip, washed with PBS, placed into complete growth medium, and photographed in phase-contrast with a Nikon microscope (Nikon Diaphot 300). Matched-pair marked wound regions were photographed again after 6 and 18 h.

Data analysis. All experiments were performed in at least three independent assays. Data are summarized as means ± standard deviations. Statistical analysis of the results was performed by Student's t test for unpaired samples. A P value of <0.05 was considered statistically significant.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

 
Murine fibroblasts release sAxl. Murine L929 fibrosarcoma cells abundantly express Axl mRNA and protein, as detected by RT-PCR and Western blotting, whereas the amount of Axl is higher in a TNF--resistant derivative of the L929 cell line referred to here as L929R (Fig. 1A and B). Membrane-bound Axl could also be detected on the cell surface of both fibroblast cell lines by flow cytometry (Fig. 1C) and confocal microscopy (data not shown). Therefore, we have chosen these two cell lines as model systems for analysis of the mechanism(s) of sAxl generation and comparison. To investigate whether these cells release sAxl into the culture medium, conditioned medium was collected after 18 h of culture. Next, sAxl was immunoprecipitated from the conditioned medium with specific Abs and immunoprecipitates were analyzed by Western blotting. In parallel, the amount of Axl in the cell lysates was assessed. Indeed, L929 fibroblasts constitutively released sAxl into the culture medium, as shown by the ability of anti-Axl Abs to precipitate a characteristic 65-kDa sAxl isoform (Fig. 1D), which is in accord with previous findings (23). Further, a full-length Axl protein (120 kDa) was detected in the cell lysates (Fig. 1D), whereas isotype-matched control Abs did not precipitate Axl (data not shown). To assess whether sAxl is glycosylated, the immunoprecipitates from the conditioned medium were treated with N-glycosidase and the resulting products were analyzed by Western blotting. As shown in Fig. 1E, the treatment of sAxl with N-glycosidase leads to a shift of the specific band to a lower molecular mass position (about 60 kDa), which presumably corresponds to a nonglycosylated form of this molecule.

View larger version (44K): [in this window] [in a new window]   FIG. 1. Membrane-bound Axl and sAxl are present in L929 and L929R fibroblasts. (A) RT-PCR analysis of Axl expression in L929 and L929R cells. Amplification of the ß-actin message was used to normalize the amount of cDNA. (B) L929 and L929R cells were lysed, and expression of Axl was analyzed by Western blotting with specific Abs. Lysates from Axl–/– fibroblasts were used as a negative control. Expression of ß-actin was detected on the same membrane after stripping and served as a loading control. (C) Expression of Axl on the cell membrane of L929 and L929R fibroblasts was assessed by flow cytometry analysis. (D) sAxl was detected in cell-conditioned medium (CM), and membrane-bound Axl was detected in lysates (L) from L929 and L929R cells by Western blotting after immunoprecipitation with specific anti-Axl Abs. (E) Glycosylation pattern of sAxl. sAxl was immunoprecipitated from cell-conditioned medium and treated with N-glycosidase or left untreated, as described in Materials and Methods. After treatment, protein lysates were analyzed by Western blotting with anti-Axl Abs.

View larger version (39K): [in this window] [in a new window]   FIG. 2. Regulation of Axl shedding. L929 (A) and L929R (B) cells were treated with 200 ng/ml of PMA for different times, and the concentration of sAxl in cell-conditioned medium was evaluated by a specific ELISA. Untreated cells were used as controls. *, P < 0.05 versus control samples. L929 (C) and L929R (D) cells were left untreated or treated with PMA for 2 h. Expression of membrane-bound Axl was evaluated by flow cytometry. (E and F) Cells were treated with PMA (200 ng/ml), Gas6 (50 ng/ml), IL-15 (50 ng/ml), TNF- (10 ng/ml), and LPS (10 ng/ml) for 2 h, and the concentration of sAxl in the culture medium was quantified by ELISA. Untreated (medium) cells were used as controls. **, P < 0.01 versus control samples.

Metalloproteinase inhibitors block constitutive and inducible Axl shedding. It has been reported that both human and murine Axl proteins undergo proteolytic cleavage by an as yet unidentified protease(s) to yield soluble variants of this molecule (23, 50). Members of the metalloproteinase superfamily have been shown to be responsible for the cleavage of the majority of shed proteins (14). The proteolytic activity of metalloproteinases can be blocked by broad-spectrum metalloproteinase inhibitors such as batimastat or GM6001 (1). To test whether the release of sAxl is mediated by metalloproteinases, cells were first incubated with GM6001 or its inactive analog as a control. These experiments demonstrated the ability of GM6001 to suppress constitutive (2.8- and 3.5-fold, respectively) and PMA-induced (2.9- and 3.2-fold, respectively) Axl shedding in the L929 and L929R fibroblast cell lines, compared with a control compound (Fig. 3A). Conversely, the inhibitor increased the amount of Axl in cell lysates.

View larger version (38K): [in this window] [in a new window]   FIG. 3. Effects of metalloproteinase inhibitors on Axl cleavage. L929 or L929R cells were incubated with 2.5 µM GM6001 or with its inactive analog as a control (A) or with 10 µM hydroxamate inhibitor GW280264X (B) for 1 h prior to treatment with 200 ng/ml of PMA for another 2 h. Untreated cells were used as controls. Cell-conditioned medium (CM) or cell lysates (L) were harvested and analyzed by ELISA for the presence of sAxl or membrane-bound Axl, respectively. (C) Cells were treated with the above inhibitors, followed by PMA stimulation for another 2 h. Expression of membrane-bound Axl was evaluated by flow cytometry analysis. * and **, P < 0.01 versus control samples; neg., negative.

Cleavage of Axl is reduced in murine fibroblasts lacking ADAM10 but is not affected in TACE-deficient cells. To gain further insights into the mechanism of constitutive and inducible sAxl release, MEFs generated from mouse embryos with a targeted deletion of ADAM10 or TACE were used (36, 54). The endogenous expression of Axl was rather similar in ADAM10^–/–, TACE^–/–, and respective WT MEFs, as detected by RT-PCR and Western blotting (Fig. 4A and B). The absence of ADAM10 or TACE in corresponding cells was already confirmed by Western blotting with specific anti-ADAM10 or anti-TACE Abs (18). The cells were plated in equal numbers and stimulated with PMA or left untreated, and the concentration of sAxl in the cell-conditioned medium was assessed by ELISA after 4 h, because PMA-induced release of sAxl from these fibroblasts was maximal at this time point (data not shown). These experiments demonstrated that both constitutive and PMA-inducible release of sAxl was dramatically lower in ADAM10^–/– MEFs compared with their normal WT counterparts (Fig. 4C). Notwithstanding, Axl shedding was not completely abrogated in these cells, as ADAM10^–/– MEFs constitutively released minute amounts of sAxl, whereas PMA treatment had little, if any, effect on this process (Fig. 4C). Constitutive and PMA-inducible Axl cleavage was diminished approximately 2.5- and 12.6-fold in ADAM10^–/– fibroblasts, respectively, compared with cells from ADAM10^+/+ mice. As expected, the reconstitution of ADAM10 into ADAM10^–/– MEFs (ADAM10^–/–Re) completely restored the constitutive and inducible sAxl generation. Since Axl was not proteolytically removed from the cell membrane in ADAM10-deficient fibroblasts, these cells exhibited increased expression of full-length Axl at the cell surface, as determined by staining with anti-Axl Abs and flow cytometry analysis (Fig. 4D). The requirement of ADAM10 for sAxl generation was further confirmed in at least two independently derived ADAM10-deficient MEFs (data not shown). No significant changes in sAxl production were observed in TACE^–/– versus TACE^+/+ MEFs. It should, however, be noted that the amount of constitutively released sAxl was slightly higher in fibroblasts from TACE^+/+ and TACE^–/– mice compared with ADAM10^+/+ and ADAM10^–/– MEFs, while PMA-inducible cleavage was somewhat reduced (Fig. 4C). This fact may indicate that the absence of TACE attenuates PMA-inducible shedding of Axl to a certain extent but cannot considerably affect this process.

View larger version (41K): [in this window] [in a new window]   FIG. 4. Analysis of sAxl release in ADAM10- or TACE-deficient MEFs. Expression of Axl in different MEFs was assessed by RT-PCR (A) and Western blotting (B). Amplification of the ß-actin message was used to normalize the amount of cDNA to be used. Detection of ß-actin protein was used to prove equal loading of cell lysates. (C) MEFs were treated with 200 ng/ml of PMA for 4 h, and the sAxl concentration in the culture medium was detected by ELISA. Untreated cells were used as a control. **, P < 0.05 versus ADAM10+/+ cells; ***, P < 0.01 versus untreated samples. (D) Expression of membrane-bound Axl on ADAM10+/+ and ADAM10–/– MEFs was evaluated by flow cytometry. (E and F) L929 and L929R cells were transfected with ADAM10 or scrambled (control) siRNA oligonucleotides, and expression of ADAM10 was assessed by Western blotting; detection of ß-actin is shown as a loading control (E). (F) Forty-eight hours after transfection, cells were treated with PMA for 2 h or left untreated. Next, the concentration of sAxl in cell-conditioned medium was evaluated by ELISA. *, P < 0.05; **, P < 0.01 (versus cells transfected with scrambled control oligonucleotides). The data represent at least three separate experiments with comparable results.

The membrane-proximal sequence of Axl is important for shedding. To identify a potential ADAM10 cleavage site, we performed a deletion analysis whereby three partially overlapping 14-aa stretches in the membrane-proximal region of Axl were removed (Fig. 5A). Given that cleavage of human Axl was mapped to the 14-aa stretch in the extracellular region (50), the first deletion mutant (Axl1) corresponded to the homologous sequence in mouse Axl. The resulting constructs (Axl1, Axl2, and Axl3) were transiently transfected into COS-7 cells, which have relatively high endogenous ADAM10 activity (38), and sAxl generation was assessed 48 h after transfection by ELISA. Transfection with a full-length Axl construct (Axl WT) served as a control. Expression of control and deletion constructs (Axl WT, Axl1, Axl2, and Axl3) was comparable, as detected by Western blotting (Fig. 5B). As demonstrated in Fig. 5C, transfection with Axl1 decreased constitutive and PMA-inducible sAxl release about twofold. Spontaneous and inducible generation of sAxl was considerably lower in cells transfected with the Axl2 (4.9- and 5.1-fold, respectively) and Axl3 (7.1- and 8.2- fold, respectively) mutants. Taken together, these results indicate that deletions in the membrane-proximal region of Axl dramatically affect ADAM10-mediated sAxl generation.

View larger version (22K): [in this window] [in a new window]   FIG. 5. The membrane-proximal region of Axl is important for sAxl generation. (A) Axl deletion mutants were generated as described in Materials and Methods. COS-7 cells were transiently transfected with full-length Axl (Axl WT) or with Axl deletion mutants (Axl1, Axl2, and Axl3) lacking different 14-aa sequence in the membrane-proximal region of Axl. FNIII, fibronectin type III; TM, transmembrane. (B) Efficiency of transfection was proved by Western blotting with anti-Axl Abs, and detection of ß-actin on the same blots is shown as a loading control. (C) After 48 h, the culture medium was replaced with fresh culture medium and the cells were incubated in the presence or absence of PMA for 1 h. Conditioned medium was collected, and the concentration of sAxl was determined by ELISA. *, P < 0.05; **, P < 0.01 (versus Axl WT-transfected cells). The results are representative of three independent experiments.

View larger version (41K): [in this window] [in a new window]   FIG. 6. Detection of sAxl, Mer, and Tyro3 in culture medium from DCs and tumor cell lines. (A) DCs were generated as described in Materials and Methods, and expression of Axl, Mer, and Tyro3 on the cell membrane of WT and Axl–/– DCs was evaluated by flow cytometry analysis. (B) DCs were pretreated with GW280264X for 30 min prior to stimulation with PMA for another 4 h or left untreated. Unstimulated and Axl–/– DCs served as control cells. The concentration of sAxl or cell-associated Axl in cell-conditioned medium (CM) or cell lysates (L), respectively, and the concentrations of Mer and Tyro3 in cell-conditioned medium were analyzed by ELISA. (C) TS/A and J558 cells were incubated in the presence or absence of PMA for 4 h. Culture medium was collected, and the concentration of sAxl was evaluated by ELISA. *, P < 0.05 versus untreated cells; **, P < 0.05 versus control samples.

Thus, the constitutive and inducible release of sAxl was assessed in the cell-conditioned medium from two murine tumor cell lines, TS/A and J558L. To this end, both tumor cell lines were stimulated with PMA for 4 h or left untreated and the presence of sAxl in the cell supernatants was evaluated by ELISA. Figure 6C shows that TS/A cells constitutively produced large amounts of sAxl (0.8 to 1 ng/ml) in the culture medium, whereas PMA enhanced the release of this molecule 2.5-fold. The PMA-inducible sAxl release was associated with a reduction in the amount of cell-associated protein (data not shown). Conversely, sAxl production was considerably lower in J558L cells at the indicated time point and PMA treatment had little effect on this process (Fig. 6C), which is explained by the fact that these cells have low endogenous Axl expression, as detected by semiquantitative RT-PCR and flow cytometry analysis (see Fig. S2 in the supplemental material). Incubation of cells with the metalloproteinase inhibitor GW280264X significantly reduced both constitutive and PMA-induced Axl shedding in TS/A cells (Fig. 6C). This effect was almost undetectable in J558L cells due to the low level of sAxl generation in these cells. Taken together, these results demonstrate that sAxl is released by select murine primary and transformed cells.

sAxl is present in mouse serum. It has been reported that sAxl could be detected by immunoprecipitation with specific Abs in mouse serum, plasma, and various mouse organs, such as the brain, cerebellum, liver, and spleen (23). To confirm these results and to analyze quantitatively the amount of sAxl in mouse serum, the sera from at least five animals per strain were tested by ELISA. As shown in Fig. 7A, CH3, C57BL/6, and BALB/c mice display similar levels of circulating sAxl (range of 5 to 6 ng/ml). Next, the sAxl concentrations were assessed in sera from Axl^–/–, Axl^+/–, and WT mice (Axl^+/+). The amount of sAxl in sera from Axl^+/+ mice was comparable to that found in other strains, whereas animals heterozygous for Axl (Axl^+/–) had an approximately twofold lower concentration of sAxl (Fig. 7A). As expected, no sAxl was detectable in sera from Axl^–/– mice. It should be noted that soluble forms of Tyro3 and Mer were not present in mouse serum, as detected by specific ELISAs (Fig. S1B in the supplemental material).

View larger version (19K): [in this window] [in a new window]   FIG. 7. sAxl is present in mouse serum and associates with Gas6. (A) Sera from C57BL/6, CH3, BALB/c, Axl+/+, Axl+/–, and Axl–/– mice were tested for the presence of sAxl by ELISA. Each bar represents the mean of at least five animals per strain (*, P < 0.05; **, P < 0.01). (B) The concentration of Gas6 in mouse sera was determined by a two-site ELISA. The concentration of sAxl or Gas6 was determined by a specific ELISA for Axl or Gas6, respectively, and is shown for comparison. (C) Axl was precipitated from mouse serum with specific Abs. Immunocomplexes were subjected to SDS-PAGE and transferred onto nitrocellulose membrane, and Gas6 was detected by probing the membrane with specific Abs. Detection of Axl on the same blots served as a loading control. IgG, immunoglobulin G.

Furthermore, two other members of this family, Tyro3 and Mer, were not upregulated in DCs and MEFs from Axl^–/– animals, as assessed by RT-PCR and Western blotting (data not shown) or flow cytometry analysis (Fig. 6A and data not shown). No associations between Gas6 and Tyro3 or Mer were observed in respective two-site ELISAs (data not shown), which was not surprising given the lack of soluble forms of these receptors in mouse serum and cell-conditioned medium. This fact strongly argues that the function of the members of this RTK family is not redundant.

Axl/Gas6 complexes were also detected in the conditioned medium from L929R cells (Fig. 7B). However, we failed to detect these complexes in conditioned medium from L929 and TS/A cells, as well as DCs and MEFs from WT and Axl^–/– mice, which might be explained by the fact that these cells do not express detectable Gas6 at the mRNA and protein levels (data not shown) and thus cannot serve as a source of this protein. Taken together, these experiments show that sAxl can form heterocomplexes with Gas6 in mouse serum, which may have particular relevance for the biology of Gas6 and the ability of this ligand to mediate Gas6-specific responses.

Immobilized Axl-Fc chimeric protein promotes cell migration and induces phosphorylation of Axl and PI3K. The extracellular portion of Axl contains features which are reminiscent of cell adhesion molecules (67). It has been shown that Axl mediates cell aggregation and adhesion by homotypic-homophilic association of the extracellular domains of this molecule (9). Given that the extracellular domain of Axl can function as a specific substrate for adhesion of Axl-expressing cells (9), we next assessed in a wound-healing scratch assay whether the chimeric molecule Axl-Fc could affect the migratory properties of murine fibroblasts. Axl-Fc comprises the extracellular domain of mouse Axl (26) fused to the carboxy-terminal Fc region of human immunoglobulin G1 via a polypeptide linker. It seemed to us theoretically reasonable that the presence of the extracellular portion of Axl capable of homophilic associations might render this protein capable of mimicking effects of endogenous sAxl, thereby providing a tool to assess its function. The plates were coated with Axl-Fc or IL-3R-Fc and seeded with equal numbers of growing cells. After 18 h of culture, the cells were cleared within a defined area by scratching with a pipette tip, washed, placed into complete growth medium, photographed in phase-contrast (Fig. 8A, 0 h), and allowed to migrate into the cleared area, whereas cells cultured in the wells coated with IL-3R-Fc were used as controls. In fact, L929R fibroblasts growing in the Axl-Fc-coated wells had separated from the monolayer at the wound edges, forming visible cell aggregates, and significant numbers of these cells started to migrate into the cleared area within 6 to 18 h, compared with cells in untreated wells (data not shown) or control wells coated with IL-3R-Fc (Fig. 8). A similar effect was observed in MEFs from WT mice (Fig. 9A, right side), and in parental L929 cells, but the migratory properties of parental cells were somewhat diminished (data not shown). It should be mentioned that Axl-Fc had no effect on the growth and migratory characteristics of murine fibroblasts when added in a soluble form, and additional cross-linking with anti-Axl Abs also had no effect (data not shown). Thus, these results show that only immobilization of Axl-Fc on plastic renders this molecule biologically active to efficiently promote cell migration.

View larger version (51K): [in this window] [in a new window]   FIG. 8. Immobilized Axl-Fc chimeric protein promotes cell migration and induces the phosphorylation of Axl and PI3K. (A) L929R cells were plated onto Axl-Fc- or IL-3R-Fc (control)-coated six-well plates and allowed to grow in the presence of 10% FCS. After 18 h, a wound was created by scratching with a pipette tip (0 h). The cells were washed with PBS and incubated further to allow migration into the wounded area. Phase-contrast images of matched pairs of marked wound regions were taken 6 and 18 h later to assess cell migration. (B) L929R cells were serum starved for 4 h and incubated in Axl-Fc-coated wells for 15 min. Incubation in IL-3R-Fc (control)-coated wells or stimulation with 100 ng/ml of Gas6 was used as a negative or positive control, respectively. Cells were lysed, and Axl or PI3K was immunoprecipitated from the lysates with specific Abs. Precipitates were subjected to 10% SDS-PAGE and analyzed with anti-pTyr Abs. Detection of Axl or PI3K on the same blots was used as a loading control. The picture is representative of three independent experiments, all of which yielded highly comparable results. IP, immunoprecipitation; WB, Western blotting.

View larger version (84K): [in this window] [in a new window]   FIG. 9. Immobilized Axl-Fc chimeric protein induces cell migration and phosphorylation of Axl and PI3K in WT but not Axl–/– MEFs. (A) MEFs were plated onto Axl-Fc- or IL-3R-Fc (control)-coated six-well plates. A confluent cell monolayer was wounded by scratching with a pipette tip (0 h). The cells were washed with PBS and incubated further to allow migration into the wounded area. Phase-contrast images of matched pairs of marked wound regions were taken 6 and 18 h later to assess cell migration. (B) MEFs were serum starved for 4 h and incubated in Axl-Fc-coated wells for 15 min. Incubation in IL-3R-Fc-coated (control) wells or stimulation with 100 ng/ml of Gas6 was used as a negative or positive control, respectively. Cells were lysed, and Axl or PI3K was immunoprecipitated from the lysates with specific Abs. Precipitates were subjected to 10% SDS-PAGE and analyzed with anti-pTyr Abs. Detection of Axl or PI3K on the same blots was used as a loading control. IP, immunoprecipitation; WB, Western blotting.

Remarkably, the migratory properties of MEFs from Axl^–/– mice were dramatically reduced compared with those of control WT cells (Fig. 9A). This was already detectable after 6 h of incubation, whereas at 18 h total wound closure was observed in Axl-Fc-coated wells seeded with MEFs from WT animals. In contrast, the migratory characteristics of Axl^–/– fibroblasts were almost undistinguishable in Axl-Fc-coated versus IL-3R-Fc-coated (control) wells, in which no wound closure was observed after 18 h of incubation. Moreover, the phosphorylation of transmembrane Axl and PI3K was not observed in MEFs from Axl^–/– mice (Fig. 9B), thereby providing strong support for the idea that the phosphorylation of these molecules depends on, and results from, the direct binding of immobilized Axl-Fc to membrane-bound Axl. Notably, the addition of sAxl-Fc in different concentrations (0.01 to 10 µg/ml) did not affect the ability of immobilized Axl-Fc to induce cell migration and protein phosphorylation in L929R cells and MEFs from WT mice (see Fig. S4 in the supplemental material; also data not shown).

Because L929R cells express and release Gas6, whereas sAxl-Fc binds Gas6 and neutralizes its activity (23, 69, 70), these experiments also argue against the possibility that endogenous Gas6 participates in the observed cell migration and phosphorylation events by forming a complex with immobilized Axl-Fc. In addition, immobilized Axl-Fc preserved the ability to mediate cell migration and the phosphorylation of membrane Axl and PI3K in cells treated with warfarin, which selectively inhibits posttranslational vitamin K-dependent -carboxylation of Gas6, which is essential for its receptor-binding and growth-potentiating activities (68-70) (see Fig. S4 in the supplemental material). These results indicate that endogenous Gas6 is presumably not essential for signaling- and migration-inducing effects of immobilized Axl-Fc, at least under the experimental conditions used in this study.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

 
In this study, we showed that a soluble form of Axl RTK is generated through proteolytic cleavage by a disintegrin-like metalloproteinase, ADAM10. In addition, experimental evidence is provided that supports a role for immobilized sAxl in promoting cell migration and activation of membrane-bound full-length Axl and its downstream target, PI3K. Apart from the identification of ADAM10 as a major proteinase responsible for Axl ectodomain shedding, we also demonstrated that sAxl associates with endogenous Gas6 in mouse serum. A dynamic equilibrium between sAxl and Gas6 levels in biological fluids might play an important regulatory role and dramatically affect Gas6 function.

Murine primary and transformed cells spontaneously release sAxl into the culture medium, whereas PMA stimulation further enhances this process. Interestingly, murine DCs produce considerable amounts of sAxl and can serve as a source of this soluble protein. Further experiments are required to understand what role Axl and its soluble form could play in the complex biology of these antigen-presenting cells. Despite the fact that Axl cleavage was inhibited by the broad-spectrum metalloproteinase inhibitor GM6001 and an inhibitor of both ADAM10 and TACE, GW280264X, decisive evidence for the major role of ADAM10 was provided by experiments with fibroblasts derived from mice with a homozygous disruption of the ADAM10-encoding gene. Both spontaneous and inducible sAxl release was dramatically reduced in these cells compared with shedding by corresponding WT fibroblasts, whereas reconstitution of active ADAM10 expression restored Axl cleavage. Conversely, Tyro3 and Mer were not detectable in mouse serum and cell-conditioned medium, either alone or in association with Gas6, indicating a unique role for Axl among the family members.

For the members of the ADAM family, it has been suggested that structural and kinetic characteristics rather than minimal consensus shedding sequences and the identity of the amino acids constituting them regulate the access of the protease to the cleavage site (63, 66). This underlines the complexity of ADAM-substrate interactions and indicates that there may not exist a minimal consensus shedding sequence within the cleavage site but rather additional structural requirements distal from the cleavage site. The most consistent feature indicative of cleavage sites among ADAM substrates is that they usually reside in a stalk region between the membrane and an initial globular extracellular subdomain (57). The fact that sAxl generation was dramatically lower in cells transfected with Axl2 and Axl3 deletion mutants, compared with Axl1, strongly supports the idea that structural requirements play a major role in regulating the access of ADAM10 to the cleavage site of Axl.

Axl RTK is thus a novel substrate for ADAM10, although the fact that some amount of sAxl is still present in the supernatants of ADAM10^–/– cells argues that ADAM10-mediated proteolysis is not the only mechanism involved in sAxl generation. Notably, ADAM10 activity has been implicated in the constitutive shedding of a number of substrates, whereas inducible shedding is mainly attributed to TACE (14, 55). In contrast, ADAM10-deficient fibroblasts exhibited a dramatic defect in both constitutive and inducible proteolytic cleavage of Axl. Currently, we perform experiments to identify whether other members of the ADAM family may play an auxiliary role in the constitutive and/or inducible shedding of this RTK. However, a minor involvement of other protease-independent mechanisms cannot be excluded.

Ectodomain cleavage and shedding of N-glycosylated sAxl might play a particular role in distinct physiologic and/or pathological conditions and alter, in the first place, Gas6 action on the cells expressing full-length membrane Axl, as well as Tyro3 and Mer, by competing for Gas6 with the cellular receptors and inhibiting its activity. Conversely, sAxl may increase the bioavailability of Gas6 by prolonging its half-life and slowing ligand release from the heterocomplex to provide physiologically relevant levels of Gas6 in tissues, thereby resulting in local or systemic effects of this protein and influencing the nature and/or duration of the signaling event. It is also theoretically conceivable that the sAxl/Gas6 heterocomplex could bind and activate the membrane-tethered receptor. Support for this suggestion is provided by the observation that Gas6 can mediate cell aggregation by a heterotypic intercellular mechanism, whereby cell-bound Gas6 interacts with Axl on an adjacent cell (45). This mode of action is in agreement with the reported ability of soluble IL-6R to potentiate IL-6 signaling by binding to cell membrane-anchored gp130 (40). In addition, the sAxl/Gas6 complex may also be capable of interacting with transmembrane Axl through homotypic associations between Axl extracellular domains. Although initial experiments do not support a role for endogenous Gas6 in the observed ability of immobilized Axl-Fc to induce the phosphorylation of transmembrane Axl and PI3K and cell migration, additional studies are required to address this question in more detail.

Despite the fact that the exogenously added Axl ectodomain inhibits the action of Gas6 (23), it remains to be elucidated how relatively high or low circulating levels of endogenous sAxl may affect the function of Gas6. Because sAxl prevented recognition of Gas6 by monoclonal anti-Gas6 Abs in an inverted ELISA, it appears likely that sAxl is present in excess over Gas6 and all Gas6 molecules in mouse serum are presumably bound to sAxl. This may indicate that either these two molecules exist in a dynamic equilibrium or some proportion of sAxl is not associated with Gas6. Given that sAxl may also hide a certain Gas6 antigenic epitope(s) from polyclonal detection Abs, the results from the direct two-site ELISA should be interpreted with caution in regard to the actual endogenous Gas6 concentration in mouse serum.

Exogenously administered soluble IL-4R can either potentiate or inhibit the activity of IL-4 in vivo, depending on the relative molar ratios of sIL-4R to IL-4; low ratios promoted the cytokine activity, while a large excess of sIL-4 over IL-4 inhibited responses to IL-4 (56). Similarly, low levels of soluble TNF receptor presumably enhance TNF signaling, perhaps by stabilizing the ligand, whereas higher concentrations inhibit TNF activity (37). In agreement with this model, high sAxl concentrations may prevent Gas6 interaction with the membrane-bound receptors and inhibit Gas6-specific signaling, whereas low sAxl levels could potentiate Gas6 activity, but further studies are required to confirm or reject this suggestion.

Extracellular domain architectures of Axl family members resemble adhesion molecules of the cadherin and immunoglobulin superfamily and receptor-type protein tyrosine phosphatases, which were shown to promote cell adhesion through a homophilic mechanism (9). Homotypic associations involving the extracellular domains of murine Axl were also shown to mediate cell aggregation and enhance receptor phosphorylation, implicating such a mechanism in the activation of this group of RTKs and suggesting an important role in signaling cell adhesion (9). The release of the cadherin ectodomain containing homophilic binding sites is functionally of major importance for the regulation of cell adhesion and cell migration (52, 54). Thus, the ability of immobilized Axl-Fc chimeric protein to enhance cell migration and to induce, presumably through homophilic interactions, the phosphorylation of transmembrane Axl and PI3K could mimic similar effects of endogenous sAxl. Transmembrane Axl may function as a substrate adhesion molecule, mediating cell binding to proteolytically processed, immobilized Axl as a component of the extracellular matrix.

Remarkably, the adhesion between ADAM10^–/– fibroblasts is reportedly much stronger than that of their WT counterparts due to N-cadherin-mediated cell-cell adhesion (54). Given that both N-cadherin and Axl are substrates for ADAM10, the increase in the adhesive properties of these fibroblasts could also be mediated by detainment of membrane Axl. Furthermore, ADAM10-dependent cleavage of N-cadherin regulates ß-catenin nuclear signaling (54). Gas6 and Axl were also shown, through stabilization of the cytoplasmic ß-catenin pool, to have a possible role in mammary development and/or neoplastic transformation (33). Thus, Axl and N-cadherin may share not only structural but also functional similarities.

Contrary to the role of protein S as a natural anticoagulation factor, Gas6 stimulates platelets, and Gas6^–/– mice have a platelet aggregation defect that confers protection against thrombosis (4, 5). Gas6 and its receptors (Axl, Tyro3, and Mer) play an important role during thrombus formation through the ability to amplify signaling via integrin _IIbß₃ (5). Gas6 stimulates growth of cardiac fibroblasts and induces Axl-mediated chemotaxis of vascular smooth muscle cells (30, 62). Upregulated expression of Gas6 and Axl parallels neointima formation after balloon injury of the rat carotid artery (46). These facts support the important role of the Gas6/Axl system as a novel regulator of vascular cell function that may have an impact on the response of blood vessels to injury, thereby contributing to the development of atherosclerosis and/or restenosis (46).

Given that recombinant sAxl is able to bind Gas6, thereby protecting mice from life-threatening thrombosis (5), it is reasonable to suggest that the high levels of circulating endogenous sAxl observed in mouse serum in vivo may be physiologically relevant to maintain the finely tuned balance between hemostatic and antithrombotic mechanisms. The bioavailability of sAxl could have a regulatory role and provide protection against excessive Gas6 activity. It remains to be elucidated whether high or low levels of sAxl can correlate with distinct pathological conditions and serve as a prognostic marker for certain types of diseases.

Remarkably, Gas6 was not detected in serum from Axl^–/– mice, thereby indicating the existence of a certain compensatory and/or protective mechanism(s) and suggesting that Gas6 might be able to elicit harmful effects if present in a free form in the serum. Results from overexpression studies indicate that Axl is required for the secretion of Gas6 and might play an important role in cellular mechanisms regulating Gas6 expression. Further studies are necessary to test whether the amount of Gas6 may be elevated in situ in distinct pathophysiologic situations, such as the vascular injury repair process and thrombus formation, and how high circulating levels of endogenous sAxl could affect the function of Gas6 under these circumstances in vivo. Furthermore, the feasibility of using recombinant exogenous sAxl as a therapeutic agent against life-threatening thrombosis should be tested.

Many studies have documented the ability of Gas6 to support cell growth and survival (2, 10, 31). Gas6 inhibits granulocyte adhesion to endothelial cells promoted by several factors (7) and mediates cell adhesion to phosphatidylserine (49), while Mer is critical for the engulfment and efficient clearance of apoptotic cells (59). Gas6 induces through Axl STAT3-dependent mesangial cell proliferation in experimental glomerulonephritis (68-70), and both are implicated in glomerular hypertrophy at the early stages of diabetic nephropathy (47). Gas6 and Axl are also involved in the pathogenesis of rheumatoid arthritis (51). RTKs of this family play an important immunoregulatory role (42) and are essential regulators of mammalian spermatogenesis (41). Thus, a potential ability of sAxl to serve as a natural antagonist of Gas6 could have clinical relevance.

Also of importance is the fact that the extracellular domain of an RTK responsible for ligand binding reportedly plays a regulatory role in controlling receptor kinase activity, whereas deletion or truncation of this part relieves negative constraints that regulate the kinase function (50). A number of studies have provided compelling evidence for the significance of the ectodomain in regulating RTK activity by showing that in vitro deletion of this part renders many of these receptors transforming in the absence of ligand, including the epidermal growth factor receptor, the insulin receptor, and erbB2 (8, 22, 65). In accord with the fact that a number of ligands can enhance shedding of their own receptors (21, 25), Gas6 induced a modest up-regulation of sAxl release in resistant L929 fibroblasts abundantly expressing Axl on the cell surface. Thus, the proteolytic processing of Axl by ADAM10 may, at least partially, depend on, and result from, ligand binding. Importantly, the proteolytic cleavage of Axl leaves a membrane-bound carboxy-terminal fragment which is a substrate for regulated intramembrane proteolysis (RIP). The proteolytic processing and shedding of the first extracellular domain constitute a critical step in the RIP of several substrates, including Notch, amyloid precursor protein, and CD44 (28). Initial results from our laboratory suggest that Axl shedding also enhances a presenelin/-secretase-mediated RIP of the remaining cytoplasmic portion of Axl, which subsequently translocates to the nucleus (E. Bulanova et al., unpublished data).

In summary, our data demonstrate that Axl is constitutively converted into its soluble form by proteolytic cleavage and implicate ADAM10 as the metalloproteinase responsible for this RTK shedding. Rather high levels of sAxl are present in mouse serum and cell-conditioned medium from murine primary and transformed cells. Given that sAxl can form heterocomplexes with Gas6 and the ability of immobilized Axl-Fc to mediate signaling events and promote cell migration, the bioavailability of sAxl might have broad implications in diverse physiologic processes or their pathological deviations mediated by Axl itself, as well as by other members of this RTK family.

	ACKNOWLEDGMENTS

 
We are grateful to Stefan Rose-John for TACE^–/– MEFs, Dieter Adam for immortalization of Axl^–/– MEFs and for the platelet-derived growth factor receptor expression vector, Falk Fahrenholz for the bovine ADAM10 expression vector, Paola Bellosta for ARK cDNA, and Helmut Brade for LPS. We thank Martina Hein and Manuel Fohlmeister for excellent technical assistance.

This work was supported by Deutsche Forschungsgemeinschaft grant SFB415 (A10 to S.B.P. and B9 to P.S.).

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Immunology and Cell Biology, Research Center Borstel, Parkallee 22, D-23845 Borstel, Germany. Phone: 49 4537 188564. Fax: 49 4537 188403. E-mail: vbudagian{at}fz-borstel.de.

Supplemental material for this article may be found at http://mcb.asm.org/.

V.B. and E.B. contributed equally to this work.

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