TY - JOUR
T1 - MMP (matrix metalloprotease)-9-producing monocytes enable T cells to invade the vessel wall and cause vasculitis
AU - Watanabe, Ryu
AU - Maeda, Toshihisa
AU - Zhang, Hui
AU - Berry, Gerald J.
AU - Zeisbrich, Markus
AU - Brockett, Robert
AU - Greenstein, Andrew E.
AU - Tian, Lu
AU - Goronzy, Jörg J.
AU - Weyand, Cornelia M.
N1 - Funding Information:
This work was supported by the National Institutes of Health (R01 AR042527, R01 HL117913, R01 AI108906, and P01 HL129941 to C.M. Weyand and R01 AI108891, R01 AG045779, U19 AI057266, R01 AI129191, and I01 BX001669). R. Watanabe received fellowship support from the Govenar Discovery Fund. This work was partially supported by a Sponsored Research Agreement from Gilead Sciences, Inc.
Publisher Copyright:
© 2018 American Heart Association, Inc.
PY - 2018
Y1 - 2018
N2 - Rationale: Giant cell arteritis (GCA)-a primary vasculitis of medium and large arteries-is associated with vessel wall damage, elastic membrane fragmentation, and vascular remodeling. Proteinases are believed to contribute to pathogenesis by degrading extracellular matrix and causing tissue injury. Objective: The MMP (matrix metalloproteinase)-9-a type IV collagenase-is produced in the vasculitic lesions of GCA. It is unknown which pathogenic processes are MMP-9 dependent. Methods and Results: The tissue transcriptome of GCA-affected temporal arteries contained high amounts of MMP-9 transcripts, and immunostaining for pro-MMP-9 localized the enzyme to wall-infiltrating macrophages. MMP-2 and MMP-9 transcripts were also abundant in monocytes and monocyte-derived macrophages from patients with GCA. Patient-derived monocytes outperformed healthy monocytes in passing through engineered basement membranes. GCA CD (cluster of differentiation) 4+ T cells required MMP-9-producing monocytes to penetrate through matrix built from type IV collagen. In vivo functions of MMP-9 were tested in a human artery-SCID (severe combined immunodeficiency) chimera model by blocking enzyme activity with a highly specific monoclonal antibody or by injecting rMMP-9 (recombinant MMP-9). Inhibiting MMP-9 activity profoundly suppressed vascular injury, decreased the density of inflammatory infiltrates (P<0.001), reduced intramural neoangiogenesis (P<0.001), and prevented intimal layer hyperplasia (P<0.001). rMMP-9 amplified all domains of vasculitic activity, promoted assembly of T-cell infiltrates (P<0.05), intensified formation of new microvessels (P<0.001), and worsened intimal thickening (P<0.001). Systemic delivery of N-acetyl-proline-glycine-proline-a matrikine produced by MMP-9-mediated gelatinolysis-had limited vasculitogenic effects. Conclusions: In large vessel vasculitis, MMP-9 controls the access of monocytes and T cells to the vascular wall. T cells depend on MMP-9-producing monocytes to pass through collagen IV-containing basement membrane. Invasion of vasculitogenic T cells and monocytes, formation of neoangiogenic networks, and neointimal growth all require the enzymatic activity of MMP-9, identifying this protease as a potential therapeutic target to restore the immunoprivilege of the arterial wall in large vessel vasculitis.
AB - Rationale: Giant cell arteritis (GCA)-a primary vasculitis of medium and large arteries-is associated with vessel wall damage, elastic membrane fragmentation, and vascular remodeling. Proteinases are believed to contribute to pathogenesis by degrading extracellular matrix and causing tissue injury. Objective: The MMP (matrix metalloproteinase)-9-a type IV collagenase-is produced in the vasculitic lesions of GCA. It is unknown which pathogenic processes are MMP-9 dependent. Methods and Results: The tissue transcriptome of GCA-affected temporal arteries contained high amounts of MMP-9 transcripts, and immunostaining for pro-MMP-9 localized the enzyme to wall-infiltrating macrophages. MMP-2 and MMP-9 transcripts were also abundant in monocytes and monocyte-derived macrophages from patients with GCA. Patient-derived monocytes outperformed healthy monocytes in passing through engineered basement membranes. GCA CD (cluster of differentiation) 4+ T cells required MMP-9-producing monocytes to penetrate through matrix built from type IV collagen. In vivo functions of MMP-9 were tested in a human artery-SCID (severe combined immunodeficiency) chimera model by blocking enzyme activity with a highly specific monoclonal antibody or by injecting rMMP-9 (recombinant MMP-9). Inhibiting MMP-9 activity profoundly suppressed vascular injury, decreased the density of inflammatory infiltrates (P<0.001), reduced intramural neoangiogenesis (P<0.001), and prevented intimal layer hyperplasia (P<0.001). rMMP-9 amplified all domains of vasculitic activity, promoted assembly of T-cell infiltrates (P<0.05), intensified formation of new microvessels (P<0.001), and worsened intimal thickening (P<0.001). Systemic delivery of N-acetyl-proline-glycine-proline-a matrikine produced by MMP-9-mediated gelatinolysis-had limited vasculitogenic effects. Conclusions: In large vessel vasculitis, MMP-9 controls the access of monocytes and T cells to the vascular wall. T cells depend on MMP-9-producing monocytes to pass through collagen IV-containing basement membrane. Invasion of vasculitogenic T cells and monocytes, formation of neoangiogenic networks, and neointimal growth all require the enzymatic activity of MMP-9, identifying this protease as a potential therapeutic target to restore the immunoprivilege of the arterial wall in large vessel vasculitis.
KW - Basement membrane
KW - Giant cell arteritis
KW - Macrophages
KW - Matrix metalloproteinases
KW - T lymphocytes
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U2 - 10.1161/CIRCRESAHA.118.313206
DO - 10.1161/CIRCRESAHA.118.313206
M3 - Article
C2 - 29970365
AN - SCOPUS:85055603208
SN - 0009-7330
VL - 123
SP - 700
EP - 715
JO - Circulation research
JF - Circulation research
IS - 6
ER -