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Inflammation Dampened by Gelatinase A Cleavage of Monocyte Chemoattractant Protein-3

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Science  18 Aug 2000:
Vol. 289, Issue 5482, pp. 1202-1206
DOI: 10.1126/science.289.5482.1202

Abstract

Tissue degradation by the matrix metalloproteinase gelatinase A is pivotal to inflammation and metastases. Recognizing the catalytic importance of substrate-binding exosites outside the catalytic domain, we screened for extracellular substrates using the gelatinase A hemopexin domain as bait in the yeast two-hybrid system. Monocyte chemoattractant protein–3 (MCP-3) was identified as a physiological substrate of gelatinase A. Cleaved MCP-3 binds to CC-chemokine receptors–1, –2, and –3, but no longer induces calcium fluxes or promotes chemotaxis, and instead acts as a general chemokine antagonist that dampens inflammation. This suggests that matrix metalloproteinases are both effectors and regulators of the inflammatory response.

Degradomics, the identification of biologically relevant substrates for the increasing number of recognized proteinases, is a challenge of proteomics. Although yeast two-hybrid screening (1) has identified intracellular protein-protein interactions, a screening rationale with a proteinase catalytic domain as target is tenuous because cleavage of library-encoded substrate would preclude detection. Therefore, to identify potential matrix metalloproteinase (MMP) substrates, we used a substrate-binding exosite domain, the hemopexin COOH-terminal (C) domain (2, 3), that is structurally and functionally distinct from the catalytic domain in a two-hybrid screen. Collagen binding by this domain of collagenolytic MMPs is a prerequisite for cleavage. Therefore, other proteins that bind to this domain may also be MMP substrates.

To determine the suitability of the two-hybrid system for extracellular proteins, we assessed the interaction between the single–disulfide-bonded gelatinase A (MMP-2) hemopexin C domain and the C domain of the tissue inhibitor of metalloproteinase–2 (TIMP-2), which contains three disulfide bonds. Deletion (4) and domain-swapping (5) studies indicate that these domains interact in the cellular activation and localization of gelatinase A to cell surface membrane type (MT)–MMPs (6). Association was detected (Fig. 1, A and B), indicating that in yeast at 30°C, a stable, functional protein fold in domains that normally contain disulfide bonds was achieved.

Figure 1

MCP-3 interactions with the gelatinase A hemopexin C domain (Hex CD). (A) In the yeast two- hybrid assay only the yeast transformants Hex CD/TIMP-2 CD, Hex CD/MCP-3, and p53/SV40 (positive control) showed growth on medium lacking histidine. (B) β-Galactosidase levels in yeast expressing the indicated fusion proteins. (C) Cross-linking of MCP-3 and recombinant hemopexin C domain. MCP-3 alone, or in the presence of 0.5 M equivalent (+), 1.0 M equivalent (++), or 2.0 M equivalents (+++) of hemopexin C domain, was cross-linked with 0.5% glutaraldehyde for 20 min at 22°C. (D) ELISA binding assay of 0.5 μg of MCP-3 immobilized onto a 96-well plate and then incubated with recombinant gelatinase A hemopexin C domain or collagen binding domain (CBD).

A cDNA library was constructed from human gingival fibroblasts treated with concanavalin A (Con A), a stimulant of extracelluar matrix degradation through the activation of gelatinase A (7). Using the human gelatinase A hemopexin C domain in yeast two-hybrid screens, we identified monocyte chemoattractant protein–3 (MCP-3) as a potential binding protein (Fig. 1, A and B). MCP-3 is one of several tissue-derived CC-chemokines that recruits monocytes and other leukocytes in inflammation and osteosarcoma (8). The hemopexin C domain had a comparable interaction with both MCP-3 and the TIMP-2 C domain (Fig. 1B). Chemical cross-linking of synthetic MCP-3 to recombinant hemopexin C domain verified this interaction (Fig. 1C). The cross-linked MCP-3–hemopexin C domain had the mass of a 1:1 bimolecular complex, whereas MCP-3 alone was not cross-linked. Furthermore, the hemopexin C domain showed saturable binding to MCP-3 by an enzyme-linked immunosorbent assay (ELISA)–based binding assay (Fig. 1D). Absence of binding by recombinant gelatinase A collagen binding domain protein (9) composed of three fibronectin type II modules confirmed specificity. Full-length gelatinase A also bound MCP-3 (Fig. 2A), whereas truncated gelatinase A lacking the hemopexin C domain (N–gelatinase A) did not (Fig. 2B). No interaction was observed between gelatinase A and the related CC-chemokine, MCP-1. As controls, full-length and N–gelatinase A did bind to gelatin and TIMP-2 by the collagen binding domain and active site (10), respectively. Hence, these data demonstrate a specific requirement for the hemopexin C domain of gelatinase A for binding MCP-3.

Figure 2

Gelatinase A binding and cleavage of MCP-3. (A) Gelatin zymography of enzyme capture film assay of pro- and active gelatinase A. Five micrograms each of bovine serum albumin (BSA), gelatin, TIMP-2, MCP-1, and MCP-3 were immobilized onto a 96-well plate. Recombinant gelatinase A was then overlaid for 2 hours and the bound protein analyzed by zymography. Overlay, recombinant enzyme used. (B) Gelatin zymography as in (A), but with hemopexin C domain–truncated gelatinase A (N–gelatinase A) used as overlay. (C) Tricine gel analysis of MCP-3 cleavage by gelatinase A in the presence of equimolar amounts (relative to MCP-3) of recombinant hemopexin C domain (Hex CD), collagen binding domain (CBD), TIMP-2, or 10 μM BB-2275 (British Biotech Pharmaceuticals, Oxford, United Kingdom). (D) Tricine gel analysis of human fibroblast–mediated MCP-3 cleavage. Fibroblast cultures were treated with Con A for 24 hours at 37°C. After a 16-hour incubation with MCPs in the presence of the MMP inhibitors indicated [concentrations as in (C)], the conditioned culture media were analyzed by tricine SDS–polyacrylamide gel electrophoresis (PAGE). The masses of the MCP-3 forms in the culture media were measured by electrospray mass spectrometry. (E) Electrospray mass spectrometry, NH2-terminal Edman sequencing, and tricine gel analysis of MCP-3 cleavage products produced by recombinant gelatinase A activity. MCP-3 (5 μg) was incubated with 100 ng, 10 ng, 1 ng, 100 pg, 10 pg, 1 pg, or 100 fg of recombinant gelatinase A for 4 hours at 37°C. (F) Electrospray mass spectrometry and tricine gel analysis of MCP-1, -2, -3, and -4 after incubation with recombinant gelatinase A for 18 hours at 37°C. The NH2-terminal sequence of the MCPs is shown with the Gly-Ile scissile bond in MCP-3 in bold.

Incubation of MCP-3 with recombinant gelatinase A resulted in a small but distinct increase in electrophoretic mobility of MCP-3 on tricine gels (Fig. 2C) that was blocked by the MMP-specific inhibitor TIMP-2 and the hydroxamate inhibitor BB-2275. Exogenous recombinant gelatinase A hemopexin C domain decreased MCP-3 cleavage, whereas the collagen binding domain had no effect (Fig. 2C). In addition, thek cat/K m decreased from 8000 M−1 s−1 for full-length gelatinase A cleavage of MCP-3 to 500 M−1 s−1 for N–gelatinase A, confirming the mechanistic importance of the hemopexin C domain exosite in MCP-3 degradation. These kinetic parameters for full-length gelatinase A cleavage of MCP-3 were higher than for denatured type I collagen (gelatin), 7580 M−1s−1 (11), indicating that MCP-3 should be efficiently cleaved in vivo. Indeed, MCP-3 but not MCP-1 was cleaved by cultured human fibroblasts after Con A–induced gelatinase A activation (Fig. 2D). Cleavage of MCP-3 by other MMPs was also examined (12). Although gelatinase A was the most efficient of these proteinases, collagenase-3 (MMP-13) and MT1-MMP (MMP-14) also processed MCP-3, further favoring the cleavage of MCP-3 in vivo. However, MCP-3 was not a general MMP substrate because matrilysin (MMP-7), which lacks a hemopexin C domain, and the leukocyte MMPs—collagenase-2 (MMP-8) and gelatinase B (MMP-9)—did not cleave MCP-3.

To identify the cleavage site in MCP-3, we performed electrospray mass spectroscopy. The mass of the gelatinase A–cleaved MCP-3 was 8574 daltons both in vivo (Fig. 2D) and in vitro (Fig. 2, C and E), a reduction from the mass of the full-length molecule (8935 daltons) by the exact mass of the NH2-terminal four residues. NH2-terminal Edman sequencing confirmed the scissile bond to be Gly4-Ile5 (Fig. 2E), a preferred sequence for gelatinase A cleavage (13) that is absent in other MCPs not cleaved by gelatinase A (Fig. 2F), including mouse MCP-3 (12).

A monoclonal antibody to human MCP-3 coimmunoprecipitated progelatinase A, but not the active enzyme, from the synovial fluid of an arthritis patient (Fig. 3A). Full-length MCP-3 was identified in these immunocomplexes with an affinity-purified antibody raised against the NH2-terminal five residues of MCP-3 (Fig. 3A). Gelatinase A–cleaved MCP-3 was also detected in human rheumatoid synovial fluids with affinity-purified anti-neoepitope antibody that recognizes the free amino group of the cleaved MCP-3 at Ile5, but not the full-length MCP-3 nor another truncated MCP-3 (residues 9 to 76) used as controls (Fig. 3, B and C). Hence, these data demonstrate that MCP-3 interacts with and is cleaved by gelatinase A in vivo.

Figure 3

Identification of in vivo human MCP-3–progelatinase A complexes and cleaved MCP-3(5-76) in human synovial fluid. (A) MCP-3 was immunoprecipitated with an anti-MCP-3 monoclonal antibody from 200 μl of synovial fluid of a patient with seronegative spondyloarthropathy. Gelatin zymography (top) and Western blotting with rabbit anti-MCP-3(1-76) (bottom) of the complexes. (B) Characterization of affinity-purified antibody raised against residues one to five of MCP-3 [anti-(1-76)] and the neoepitope at residues five to nine of MCP-3 [anti-(5-76)]. (C) Identification of MCP-3(5-76) in human rheumatoid synovial fluid. Total protein is shown after SDS-PAGE and Coomassie staining. Detection of full-length and gelatinase A–cleaved forms of MCP-3 in human synovial fluid by Western blotting with antibodies as indicated. Control blot indicates anti-(5-76) preadsorbed with synthetic MCP-3(5-76) before use.

MCP-3 binds leukocyte CC-receptor–1 (CCR-1), –2, and –3 and mobilizes intracellular calcium, resulting in directed cell migration of leukocytes. NH2-terminal truncation of synthetic MCP-1 and MCP-3 at different sites has variable effects on their agonist activity (14, 15). Gelatinase A–mediated removal of the first four residues of MCP-3 resulted in the loss of CCR-1 and -2 activation in THP-1 cells (16), a monocyte cell line that expresses these two receptors. Neither gelatinase A–cleaved MCP-3 in the presence of 1/1000 (mole ratio) gelatinase A (Fig. 4A) nor synthetic MCP-3(5-76) (MCP-3 residues 5 to 76, corresponding to the gelatinase A–cleaved form) (Fig. 4B) elicited a calcium response. In addition to loss of CCR agonist activity, MCP-3(5-76) antagonized the subsequent response not only to MCP-3, but also to MCP-1 (Fig. 4B) and macrophage inflammatory protein–1α (MIP-1α) (17). MCP-1 only binds CCR-2 and MIP-1α binds to CCR-1 and CCR-5, confirming the CCR-1 and CCR-2 antagonist activity of MCP-3(5-76). MCP-3(5-76) did not block the calcium response to macrophage-derived chemokine (MDC), which binds CCR-4, a receptor not bound by MCP-3 (Fig. 4B). The physiological relevance of MCP-3 antagonism was confirmed by cell-binding assays (18). Scatchard analysis showed that synthetic MCP-3(5-76) bound THP-1 cells with high affinity [dissociation constant (K d) = 18.3 nM], similar to that of full-length MCP-3 (K d = 5.7 nM) (Fig. 4C). In transwell cell migration assays (19), MCP-3(5-76) was not chemotactic, even in amounts 100-fold higher than full-length MCP-3 (Fig. 4D). MCP-3(5-76) also functioned as an antagonist in a dose-dependent manner to inhibit the chemotaxis directed by full-length chemokine (Fig. 4D). Thus, MMP inactivation of MCP-3 also generates a broad-spectrum antagonist for CC-receptors that retains strong cellular binding affinity and modulates the response to a number of related chemoattractants.

Figure 4

Cellular responses to gelatinase A– cleaved MCP-3. (A) Loss of intracellular calcium mobilization by MCP-3 after gelatinase A cleavage. Fluo-3AM–loaded THP-1 monocytes were treated (arrows) with 5 nM MCP-3 or MCP-1 (top scans) or the respective chemokine incubated first with gelatinase A for 18 hours (bottom scans). The data are presented as relative fluorescence emitted at 526 nm. (B) Intracellular calcium mobilization by MCP-3, MCP-1, and MDC. Fluo-3AM–loaded THP-1 monocytes or a B-cell line transfected with CCR-4 (for MDC) were first exposed to either 0 nM (left arrow, top scans) or 500 nM MCP-3(5-76) (left arrow, bottom scans), followed by MCP-3 (30 nM), MCP-1 (5 nM), or MDC (5 nM), as indicated (right arrow, top and bottom scans). (C) THP-1 cell receptor binding of MCP-3 and MCP-3(5-76). (D) Transwell assay of monocytes treated with MCP-3 and MCP-3(5-76) at the indicated amounts.

To examine the biological effects of gelatinase A cleavage of MCP-3 in inflammation, we injected various mole ratios of full-length MCP-3 and gelatinase A–cleaved or synthetic MCP-3(5-76) into mice subcutaneously (20). Full-length, but not cleaved MCP-3, induced infiltration of mononuclear inflammatory cells with associated matrix degradation at 18 hours after injection (Fig. 5, A to D). A statistically significant reduction in the mononuclear cell infiltrate in response to as little as a 1:1 mixture of MCP-3(5-76) with MCP-3 was observed (Fig. 5E). In a separate mouse model of inflammation, the cellular infiltrate in 24-hour zymosan A–induced peritonitis (21) was attenuated after intraperitoneal injection with MCP-3(5-76). Consistent with morphometric examination of the cell content in the peritoneal cavity (Fig. 5, F and G), flow cytometric analysis (22) of peritoneal washouts showed that macrophage (F4/80+) cell counts were reduced by ∼40% at both 2 and 4 hours after MCP-3(5-76) treatment (Fig. 5, F and G).

Figure 5

Animal responses to gelatinase A–cleaved MCP-3. Light micrographs of H&E-stained subcutaneous tissue sections (tissue region as shown) of mice injected with (A) saline/buffer control M, muscle; A, adipocyte; C, loose connective tissue. Bar, 20 μm., (B) MCP-3, (C) gelatinase A–cleaved MCP-3, or (D) 2:1 molar ratio of gelatinase A– cleaved MCP-3:full-length MCP-3. (E) After subcutaneous injections with MCP-3 and MCP-3(5-76) mixtures, the infiltrating mononuclear cells were enumerated and expressed as cells per 75,000 μm2(n = 5, mean ± SD; P < 0.01 compared with MCP-3). (F and G) H&E-stained cytospins of intraperitoneal washouts of zymosan A–treated mice injected 24 hours later with (F) MCP-3(5-76) or (G) saline for 4 hours. Macrophage cell counts by flow cytometric analysis for each group of mice are presented below (n = 5, mean ± SD;P < 0.05 by analysis of variance).

Chemokine inactivation and clearance in vivo is not well understood (23). Although several examples are known in which metalloproteinase activity activates cytokines (24) and α-defensins (25), this study demonstrates the extracellular inactivation of a cytokine in vivo by MMP activity. The relative amounts of intact and cleaved MCP-3 that are present after pathophysiological cleavage regulate chemotaxis and the extent of inflammation. Identification of the importance of gelatinase A in the pathophysiological processing of MCP-3 reveals the intersection of two distinct pathways that regulate the extracellular environment and the immune response. MMP expression is induced at foci of inflammation by leukocytic and stromal-derived cytokines. Notably, gelatinase A is derived largely from stromal cells and is not usually expressed by leukocytes (26); these cells express MMP-8 and gelatinase B, both of which do not cleave MCP-3. Therefore, leukocyte proteolytic activity is unlikely to disrupt cognate chemokine gradients. Overall, the activity of several tissue-derived MMPs, and gelatinase A in particular, can contribute to the cessation of the host response, an important aspect of healing and tissue resolution. Because TGF-β1, a growth factor that orchestrates wound repair (27), stimulates gelatinase A but represses other MMPs (28), the interactions of MMPs with chemokines provide a self-attenuating network to dissipate proinflammatory activities. Therefore, MMPs are both effectors and regulators of inflammation.

  • * To whom correspondence should be addressed. E-mail: overall{at}interchange.ubc.ca

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