Recognition Versus Adaptive Up-regulation and Degradation of CC Chemokines by the Chemokine Decoy Receptor D6 Are Determined by Their N-terminal Sequence*

The chemokine decoy receptor D6 controls inflammatory responses by selective recognition and degradation of most CCR1 to CCR5 agonistic ligands. CCL14 is a homeostatic chemokine present at high concentrations in the serum with a weak agonist activity on CCR1. Under inflammatory conditions, plasmin and UPA-mediated truncation of 8 amino acids generates the potent CCR1/CCR3/CCR5 isoform CCL14(9–74), which is further processed and inactivated by dipeptidyl peptidase IV/CD26 that generates CCL14(11–74). Here we report that D6 efficiently binds both CCL14 and its truncated isoforms. Like other D6 ligands, the biologically active CCL14(9–74) induces adaptive up-regulation of D6 expression on the cell membrane and is rapidly and efficiently degraded. In contrast, the D6-mediated degradation of the biologically inactive isoforms CCL14(1–74) and CCL14(11–74) is very inefficient. Thus, D6 cooperates with CD26 in the negative regulation of CCL14 by the selective degradation of its biologically active isoform. Analysis of a panel of CC chemokines and their truncated isoforms revealed that D6-mediated chemokine degradation does not correlate with binding affinity. Conversely, degradation efficiency is positively correlated with D6 adaptive up-regulation. Sequence analysis indicated that a proline residue in position 2 of D6 ligands is dispensable for binding but crucial for D6 adaptive up-regulation and efficient degradation.

The chemokine system is composed by nearly 50 ligands that exert chemotactic and cytokine-like activities through the binding to 18 G protein-coupled receptors (1)(2)(3). Chemokines can be classified according to the number and relative position of cysteine residues in the N terminus into four classes (C, CC, CXC, and CX3C). Alternatively, they may also be classified on the basis of their expression patterns and functions as "inflammatory" (produced only upon activation) and "homeostatic" (expressed in discrete locations in the absence of apparent activating stimuli) (4). In addition to gene expression regulation, post-transcriptional regulatory mechanisms, including chemokine degradation by non-signaling chemokine decoy receptors (5,6), binding to glycosaminoglycans (7), and posttranslational processing by endogenous peptidases or peptidyl arginine deiminases (8,9), are emerging mechanisms that fine tune chemokine biological activities and leukocyte recruitment.
Chemokine decoy receptors are a distinct subset of chemokine receptors characterized by their inability to transduce conventional signaling that leads to chemotaxis while supporting efficient degradation of the ligand (10). D6, the best described chemokine decoy receptor (6), is a constitutively internalizing receptor expressed by lymphatic endothelial cells (11), trophoblast cells (12), and, at lower levels, some leukocyte subsets (13). D6 selectively recognizes and degrades most inflammatory CC chemokine agonists of CCR1 to CCR5 (10). We have recently described that D6 is up-regulated on the cell membrane in a ligand concentration-dependent manner in order to optimize its scavenger performance. This adaptive up-regulation represents a rapid and unique posttranscriptional mechanism allowing D6 to control inflammation (14). In vivo experiments with D6 Ϫ/Ϫ mice have demonstrated that its chemokine scavenging activity attenuates the severity of inflammation in different experimental models (12,(15)(16)(17) and suppresses inflammation-driven tumor development (18) (19).
Chemokine extracellular processing has complex effects on the chemokine biology, in that it usually results in biological inactivation, but for some chemokines, processing increases the biological activity or receptor specificity rather then resulting in biological inactivation (8,20), and in some cases truncated molecules even act as chemotaxis antagonists in vitro and in vivo (21,22). Chemokine processing plays a unique role for a CC chemokine subfamily with an extended N-terminal domain that has to be cleaved in order to activate the molecules (23,24). This chemokine subfamily includes CCL14, CCL15, and CCL23 in humans, clustered in an identical orientation within a region spanning ϳ40 kbp of chromosome 17q11.2. Although they lack murine homologues, the murine CCL6 and CCL9 chemokines have been identified as murine orthologues of the human CCL15 and CCL23, respectively (23). The best known member of this subfamily is CCL14, also named plasmatic hemofiltrate CC chemokine 1 (25) because of its presence at high concentrations in normal human plasma (1.5-10 nM) (25). Although CCL14 shares 46% sequence identity with CCL3 and CCL4, it is a weak CCR1 agonist. Upon removal of the first 8 amino acid residues from the N terminus of CCL14 by urokinase plasminogen activator and/or plasmin, the prochemokine is converted into CCL14(9 -74), a potent agonist for CCR1, CCR3, and CCR5 (26 -28). Interestingly, the new N terminus is now recognized and processed by the dipeptidyl peptidase IV (CD26), which further cleaves 2 amino acids and generates the biologically inactive CCL14(11-74) variant (29).
To characterize the interplay between these two posttranslational regulatory mechanisms of chemokine activity, in this study we analyzed the D6 interaction properties of full-length and truncated isoforms of this subfamily of CC chemokines. Results indicate that although D6 binds the three CCL14 isoforms, it is able to efficiently degrade only the biologically active one CCL14(9 -74) that induces its adaptive up-regulation on the cell membrane. These results prompted us to reexamine recognition versus adaptive up-regulation and ligand degradation by D6 of different CC chemokines and their truncated isoforms. This analysis revealed that a proline residue in position 2 of the N-terminal domain of D6 ligands is dispensable for D6 binding but is required for high efficiency D6-mediated degradation and adaptive up-regulation.

EXPERIMENTAL PROCEDURES
Chemicals, Antibodies, and Cell Culture-Recombinant human chemokines were from R&D Systems (Minneapolis, MN), with the exception of CCL3 and CCL14(9 -74), which were purchased from Peprotech (Rocky Hill, NJ). CCL14  was obtained by incubating CCL14(9 -74) with recombinant CD26 (Sigma) in 50 mM Tris, pH 7.5, containing 1 mM EDTA. Truncation was evaluated by desalting a small aliquot on a C4 ZipTip (Millipore, Billerica, MA) and subsequent mass spectrometry on an ion trap Esquire-LC mass spectrometer (Bruker Daltonics). Once all CCL14(9 -74) was converted into CCL14 , the reaction was stopped by acidification with trifluoroacetic acid, and CCL14(11-74) was purified by liquid chromatography-mass spectrometry on a C8 Aquapore reverse phase high pressure liquid chromatography column (2.1 ϫ 220 mm; PerkinElmer Life Sciences). Edman degradation on a Procise cLC protein sequencer (Applied Biosystems, Foster City, CA) confirmed the truncation of the N terminus and was used to determine the concentration of CCL14 . CCL8 and CCL8(6 -75) were chemically synthesized or expressed in Escherichia coli, as described previously (30). 125 I-CCL4 and 125 I-CCL2 were from PerkinElmer Life Sciences. Unconjugated and phycoerythrin-conjugated rat antihuman D6 monoclonal antibodies, biotinylated goat anti-human CCL14 antibody, and the Duo Set ELISA 4 kit to measure CCL14 were purchased form R&D Systems (Minneapolis, MN). CHO-K1/hD6 and CHO-K1/mD6 transfectants, expressing human and murine D6, respectively, were obtained and cultured as previously described (15).
Binding Assays-CCL4 competitive binding was performed by incubating 3 ϫ 10 4 CHO-K1/D6 transfectants, seeded in 96-well plates the day before the experiment, with 100 pM 125 Ilabeled CCL4 in the presence of different concentrations of unlabeled CCL2, CCL4, CCL14, CCL17, or CCL22 in 60 l of binding buffer (DMEM/F-12, 4 mM HEPES, pH 7.4, and 1% BSA) at 4°C for 2 h. After incubation, the cell-associated radioactivity was measured. To estimate the K d (i.e. the equilibrium dissociation constant), CCL4 homologous competitive binding data were analyzed by non-linear regression using the equation of the homologous competitive binding curve (Prism4 software; GraphPad). Inhibition curves were analyzed using the one-site competitive binding equation to estimate the IC 50 value, from which the K i value was then calculated according to the Cheng-Prusoff equation.
Dissociation Kinetics Experiments-For ligand dissociation experiments, 3 ϫ 10 4 CHO-K1/D6 cells seeded in 96-well plates were first incubated for 3 h at 4°C with 50 pM 125 I-labeled CCL4 in 60 l of binding buffer (DMEM/F-12, 4 mM HEPES, pH 7.4, and 1% BSA). After incubation with the tracer, the unbound radioligands were removed, and the cells were washed twice with cold binding buffer. Then a 100 nM concentration of either CCL2, CCL4, CCL14, CCL17, or CCL22 was added, and the dissociation of radioactive ligand was followed. The dissociation reactions were measured over a total period of 6 h.
Receptor Internalization and Cell Surface Expression-Antibody internalization experiments were performed to evaluate D6 internalization. CHO-K1/D6 transfectants (5 ϫ 10 5 ) were washed with PBS (Biosera, East Sussex, UK) supplemented with 1% BSA (GE Healthcare Europe, Chalfont St. Giles, UK) and stained on ice with 5 g/ml anti-D6 antibody for 1 h. Labeled cells were washed and then incubated for the indicated times at 37°C in DMEM/F-12 with 1% BSA to allow receptor internalization. Where indicated, chemokines (116 nM) were added. Samples were then returned to ice, washed, and incubated with anti-rat IgG allophycocyanin for 30 min in fluorescence-activated cell sorting (FACS) buffer (PBS supplemented with 1% BSA and 0.01% NaN 3 ). To evaluate receptor up-regulation on cell the surface, cells (5 ϫ 10 5 ) were incubated at 37°C with the indicated chemokine (100 nM) for different times in DMEM/ F-12 with 1% BSA. Cells were then transferred on ice, washed, and labeled with FACS buffer containing 5 g/ml anti-D6 phycoerythrin-conjugated antibody for 1 h. For all experiments, 1 ϫ 10 4 events of viable cells were acquired using a FACS Canto flow cytometer and analyzed using the FACS Diva software (BD Biosciences).
Chemokine Scavenging Assay-CHO-K1/D6 transfectants were plated the day before the experiment in 96-well plates at a concentration of 3 ϫ 10 4 cells/well. Cells were then incubated with a 1.16 nM concentration of the indicated chemokine for increasing times. The supernatant was collected, and remaining intact chemokine was detected by sandwich ELISA or Western blot. To evaluate inhibition of chemokine scavenging, CHO-K1/D6 transfectants were plated as described above and then 4 The abbreviations used are: ELISA, enzyme-linked immunosorbent assay; DMEM, Dulbecco's modified Eagle's medium; BSA, bovine serum albumin; FACS, fluorescein isothiocyanate; PBS, phosphate-buffered saline.
incubated for 6 h in 60 l of DMEM/F-12 supplemented with 1% BSA, 0.1 nM 125 I-CCL4, and the indicated concentrations of unlabeled chemokines. Proteins in the supernatants were precipitated with 12.5% trichloroacetic acid (Carlo Erba Reagents, Rodano, Italy) at 4°C for 15 min, and both soluble and insoluble fractions were collected. The radioactivity present in each fraction was measured using a Wizard automatic counter (PerkinElmer Life Sciences). Inhibition of the degradation rate was obtained by data fitting with non-linear regression and interpolation with Michaelis-Menten equation using Prism4 software.
Statistical Analysis-Data were analyzed by unpaired Student's t test using Prism4 software. Linear regression analysis was performed, and the coefficient of correlation was calculated using Prism4 software.

Differential Interaction of CCL14 and Its Processed
Forms with D6-The chemokine decoy receptor D6 binds with high affinity most inflammatory CC chemokine agonists of CCR1 to CCR5. Three CC chemokines, namely CCL14, CCL15, and CCL23, constitute a distinct subfamily activated by proteolytic cleavage of the N terminus during inflammatory conditions. In order to understand if D6 was able to interact with this subfamily of chemokines, binding displacement experiments were performed on CHO-K1/hD6 transfectants using radiolabeled CCL4. Human D6 bound with high affinity the proteolytically activated CCL14(9 -74) isoform and with lower affinity the fulllength biologically inactive CCL14(1-74) isoform (Fig. 1A). The binding affinity of CCL14(9 -74) was in the low nanomolar range, comparable with the one of CCL4 and CCL22, whereas the calculated K i for CCL14(1-74) was similar to CCL17 (Table  1). Similar results were obtained for murine D6 (Table 1). CCL14(9 -74) is subjected to proteolytic inactivation by the dipeptidyl peptidase CD26, which further cleaves the first two amino acids from the CCL14(9 -74) N terminus, generating the biologically inactive CCL14  isoform. D6 also bound CCL14(11-74) (Fig. 1A), with a calculated K i similar to CCL14(9 -74) ( Table 1). In order to define the ability of D6 to degrade CCL14 isoforms, scavenging assays were performed. CHO-K1/hD6 transfectants were incubated with 1.16 nM CCL14(1-74), CCL14(9 -74), or CCL14(11-74) for increasing times, and the intact chemokine remaining in the supernatant was measured by ELISA. As shown in Fig. 1B, the biologically active CCL14(9 -74) was efficiently degraded by D6, whereas CCL14(1-74), although being recognized by D6, was fully recovered in the supernatant even after a 24-h incubation. Finally, the CD26-inactivated CCL14(11-74) isoform was degraded by D6 with significantly reduced efficiency as compared with CCL14(9 -74) (T1 ⁄ 2 ϭ 5.7 Ϯ 0.4 versus 2.3 Ϯ 0.2 h, respectively; p ϭ 0.0016). Because ELISA tests can detect par-tially degraded chemokines, supernatants derived from CHO-K1 or CHO-K1/hD6 incubated with CCL14(1-74) or CCL14(9 -74) for 24 h were analyzed by SDS-PAGE and Western blot. The band corresponding to CCL14(9 -74) was not detectable after incubation with CHO-K1/hD6 transfectants, indicating complete degradation of the protein, whereas the band corresponding to CCL14(1-74) was not affected by incubation with either CHO-K1 or CHO-K1/hD6 transfectants, consistent with a lack of degradation by D6 (Fig. 1C). These data identify CCL14 and its processing isoforms as new D6 ligands and indicate that CCL14 processing not only affects its biological properties but also influences its binding affinity for D6. Furthermore, since cleavage of the first 2 amino acids from CCL14(9 -74) does not influence D6 binding but significantly impairs D6-mediated degradation, these results also indicate that a direct correlation between ligand affinity and degradation by D6 is not present for CCL14 and its truncated isoforms.
Lack of D6 Interaction with CCL15, CCL23, and Their Truncated Isoforms-Like CCL14, CCL15 and CCL23 are also produced as prochemokines that undergo proteolytic cleavage of the N terminus during inflammatory conditions to be activated. Differently from CCL14, no binding was detected on CHO-K1/ hD6 transfectants for CCL15 and CCL23, both for full-length and truncated isoforms ( Fig. 2A). Similarly, CHO-K1/mD6 transfectants were unable to bind both full-length and truncated isoforms of CCL6 and CCL9, the murine CCL15 and CCL23 orthologues (23) (Fig. 2B).
CCL14(1-74) Is Not a D6 Antagonist-Since CCL14(1-74) is recognized by D6 but not degraded, we asked whether this chemokine isoform might work as a D6 antagonist. To this purpose, we first evaluate whether CCL14(1-74) could modify the constitutive internalization of D6 by performing antibody internalization experiments. CHO-K1/hD6 transfectants were incubated at 4°C in the presence of a monoclonal antibody to D6 in order to label only receptors on the cell surface and were then returned at 37°C for increasing times in the presence of CCL14(1-74) or CCL14(9 -74). As shown by Fig. 3A, the D6 constitutive internalization rate was not modified by the addition of different CCL14 isoforms, suggesting that these chemokine isoforms, like the other D6 ligands, could not influence the receptor internalization rate. Since inflammatory CC chemokines are able to adaptively up-regulate D6 surface expression levels (14), we investigated whether different CCL14 isoforms could exert a similar effect. As shown in Fig. 3B, although CCL14(9 -74) was able to induce a dose-dependent increase of D6 expression to a similar extent as other D6 high affinity ligands, including CCL3L1, CCL4, and CCL17, CCL14(1-74) did not modify D6 surface levels. These data were confirmed by immunofluorescence experiments on CHO-K1/ hD6 transfectants (Fig. 3E). CCL14(9 -74) like CCL22 was able   1-74) addition, whereas co-incubation with CCL14(9 -74), CCL17, or CCL22 inhibited CCL4 degradation rate (Fig. 3C). To further investigate the potential inhibitory activity of CCL14(1-74) on D6 scavenging, dissociation curves were performed using radiolabeled CCL4 at the equilibrium (3 h) on CHO-K1/hD6 transfectants and subsequently incubating cells for increasing times with unlabeled chemokines. 125 I-CCL4 was fully displaced from the receptor by the homologous unlabeled chemokine (Fig. 3D). Heterolo-gous dissociation reactions indicate that 125 I-CCL4 could also be fully displaced from the receptor by unlabeled CCL17, CCL22, and CCL14(9 -74), with dissociation curves similar to those observed with homologous dissociation. On the contrary, CCL14(1-74) was unable to fully displace 125 I-CCL4, suggesting that it has only partially overlapping binding sites on D6.
The N Terminus Dictates the Interaction and Fate of D6 Ligands-Results reported above indicate that the biological outcome of D6 binding to CCL14 and its processing isoforms is strongly influenced by the N-terminal domain of the ligand. Other chemokine isoforms with a modified N-terminal domain were tested in binding and scavenging assays on CHO-K1/hD6 transfectants to understand whether this also applies to other D6 ligands. CCL3 is a non-allelic isoform of CCL3L1 with reduced agonistic activity on CCR5 and decreased binding affinity for both CCR5 and D6 due to only a few amino acid substitutions, including the presence of a serine instead of a proline residue at position 2 (31). CCL3 displaced 125 I-CCL4 with a calculated K i similar to CCL14(1-74) (Fig. 4A), it was degraded by D6-expressing cells with a significantly reduced efficiency as compared with CCL3L1 (T1 ⁄2 ϭ 6.3 Ϯ 0.3 versus 0.5 Ϯ 0.1 h, respectively; p ϭ 0.0006) (Fig. 4, B and C), it did not induce D6 membrane up-regulation (Fig. 4, E and F), and it only partially displaced previously bound CCL4 (Fig. 4D). These data indicate that the N-terminal proline residue in position 2 of CCL3L1 is required to modify receptor trafficking that leads to rapid chemokine degradation. When the processed isoform of CCL3, CCL3(5-68) (20), was tested, it was found to bind D6 with higher binding affinity, as compared with CCL3 ( Fig. 4A and Table 1), but was not degraded by D6-expressing cells (Fig. 4, B and C), did not modify D6 surface expression levels (Fig. 4,  E and F), and only partially displaced previously bound CCL4 (Fig. 4D).
These data indicate that the N-terminal portion of CCL3 is not required for D6 binding. On the contrary, deletion of the first 4 amino acids of CCL3 increased its binding affinity to D6 but completely abolished its degradation. Finally, when CCL8 and its truncated isoform CCL8(6 -75) (30) were tested in D6 binding and scavenging experiments, N-terminal truncation of CCL8 did not significantly affect D6 binding (Table 1), but CCL8 (6 -75) was degraded with a significantly reduced effi-ciency as compared with full-length CCL8 (T1 ⁄ 2 ϭ 6.4 Ϯ 0.4 versus 2.5 Ϯ 0.1 h, respectively; p ϭ 0.003), similar to CCL3 and CCL14(11-74) (data not shown). Binding, Adaptive Up-regulation, and Degradation of Different D6 Ligands-Results reported above indicate that D6 ligands can be classified into three classes according to degradation efficiency: 1) chemokines degraded with high efficiency (including CCL14(9 -74) as well as CCL2, CCL3L1, CCL4, and CCL22); 2) chemokines degraded with low efficiency (including CCL14  and CCL8(6 -75) as well as CCL3); and 3) chemokines that are not degraded (including CCL14(1-74) and CCL3 (5-68)). For the chemokines evaluated in this study, no direct correlation was found between binding affinities and degradation efficiency (Fig. 5A), indicating that chemokine recognition by D6 does not necessarily result in its efficient degradation. On the other hand, only chemokines that are degraded with high efficiency are also able to modify intracellular D6 traffic, as shown by the positive correlation between chemokine degradation efficiency and D6 adaptive up-regulation on the cell membrane (Fig. 5B). Finally, a strong correlation was found between chemokine degradation efficiency and displacement of CCL4 previously bound to D6 (Fig. 5C), indicating that only chemokines with D6 overlapping binding sites with CCL4 are able to induce their rapid degradation. Interestingly, sequence analysis ( Fig. 6) revealed that all members of this class of D6 ligands, with the only exception of CCL17, have a proline residue in position 2, suggesting a relevant role for this amino acid in the induction of D6 adaptive redistribution on the cell membrane that results in efficient chemokine degradation.

DISCUSSION
Protease-mediated processing and decoy/scavenger receptors are emerging as key regulatory mechanisms tuning the biological activity of chemokines during inflammatory responses (5,8). CCL14, CCL15, and CCL23 represent a unique subfamily of chemokines, in that they are classified as constitutive because they circulate at substantial levels in the serum of healthy subjects but act as inflammatory chemokines after cleavage of their unique N-terminal domain (23). This study identifies one of these chemokines, namely CCL14, and its truncated isoforms as new ligands for the chemokine decoy receptor D6. Unexpectedly, although it was recognized with similar affinity, the scavenging activity of D6 for the three CCL14 isoforms is completely different. The full-length biologically inactive CCL14(1-74) is not degraded by D6, whereas D6 degrades the inflammatory chemokine CCL14(9 -74) with high efficacy, and its efficacy is significantly reduced for the CD26-inactivated CCL14  isoform. Thus, the N-terminal portion of CCL14, which controls the biological activity of this chemokine, also plays a key role in its degradation. Removal of the first 8 amino acids is required for CCL14 conversion into a potent inflammatory chemokine but also allows D6-mediated degradation, and further proteolytic cleavage strongly impairs its biological activity and similarly reduces the rate of degradation via D6. D6 may thus be added to the regulatory mechanisms of CCL14 activity. CCL14 is present in the blood as an inactive chemokine. It is proteolytically activated by serine proteases of the fibrinolytic cascade to a potent chemoattractant for CCR1/ CCR3/CCR5-expressing cells (26) and is then either further processed by CD26 or degraded by the scavenging receptor D6 (Fig. 7).
Processing of CCL14(9 -74) to CCL14(11-74) strongly affects the efficiency of D6-mediated degradation. This conversion is mediated by CD26, a dipeptidyl peptidase that cleaves specifically after a proline residue present in position 2 of CCL14 (9 -74). In order to test the relevance of this residue for D6-mediated degradation, we compared CCL3L1 with its nonallelic isoform CCL3, which only differs by a proline-to-serine substitution in position 2 (31), and its truncated isoform CCL3(5-68). As compared with CCL3L1, both CCL3 and CCL3(5-68) showed a significant reduction of D6-mediated degradation. Similarly, the CCL8 truncated isoform CCL8(6 -75) retained binding to D6, but it was degraded at a significantly slower rate as compared with CCL8. Collectively, these data indicate that there is no correlation between chemokine binding affinities and their effective degradation by D6 and that a proline residue in position 2 of the N-terminal domain of D6 ligands is required for rapid degradation.
Results presented here describe CCL14(1-74) as the first D6 ligand that is not degraded. CCL14(1-74) also did not affect D6 constitutive internalization or membrane up-regulation; nor did it modify inflammatory degradation of other ligands. For these characteristics, CCL14(1-74) may be considered the first D6 neutral ligand (32). Heterologous dissociation curves indicated that unlabeled CCL14(1-74) only partially displaced previously bound 125 I-CCL4 (Fig. 3), suggesting that it interacted with D6 regions that are not available when the receptor is occupied with other ligands or that it had partly overlapping D6 binding sites. The same behavior in dissociation experiments was found for CCL3 and CCL3(5-76). Interestingly, a similar phenomenon was observed for other chemokine receptors, such as CCR1 (33), CXCR2 (34), and the virus-encoded ORF74 and US28 chemokine receptors (32).
Chemokine interaction with their cognate receptors is believed to occur through a first interaction of the rigid loop of the chemokine that follows the second cysteine, which is important for high affinity binding, followed by the interaction of the flexible N terminus of the chemokine preceding the first cysteine, which is essential for the subsequent receptor activation (35). We are here proposing that a similar mechanism may also occur for the chemokine decoy receptor D6, in which chemokines may first bind D6 with their N-loop and then activate their pathway to degradation through the binding of their N-terminal proline to the D6 seven-transmembrane bundle. In the absence of this second step, as in the case of ligands without a proline in position 2, receptor trafficking is not modified, and the D6-dependent degradative activity is strongly reduced.
In conclusion, results presented here indicate that D6 cooperates with CD26/dipeptidyl peptidase IV (29) in the inactivation and degradation of biologically active CCL14 isoforms. Moreover, by using CCL14 and other chemokine isoforms, we have shown that a proline residue in position 2 of D6 ligands is dispensable for receptor binding, but it is required to induce receptor traffic modifications resulting in efficient degradation of inflammatory CC chemokines.