Periodontal-induced chronic inflammation triggers macrophage secretion of Ccl12 to inhibit fibroblast-mediated cardiac wound healing
Kristine Y. DeLeon-Pennell, Rugmani Padmanabhan Iyer, Osasere K. Ero, Courtney A. Cates, Elizabeth R. Flynn, Presley L. Cannon, Mira Jung, De’Aries Shannon, Michael R. Garrett, William Buchanan, Michael E. Hall, Yonggang Ma, Merry L. Lindsey
Kristine Y. DeLeon-Pennell, Rugmani Padmanabhan Iyer, Osasere K. Ero, Courtney A. Cates, Elizabeth R. Flynn, Presley L. Cannon, Mira Jung, De’Aries Shannon, Michael R. Garrett, William Buchanan, Michael E. Hall, Yonggang Ma, Merry L. Lindsey
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Research Article Cardiology Inflammation

Periodontal-induced chronic inflammation triggers macrophage secretion of Ccl12 to inhibit fibroblast-mediated cardiac wound healing

Abstract

Chronic inflammatory diseases, such as periodontal disease, associate with adverse wound healing in response to myocardial infarction (MI). The goal of this study was to elucidate the molecular basis for impaired cardiac wound healing in the setting of periodontal-induced chronic inflammation. Causal network analysis of 168 inflammatory and extracellular matrix genes revealed that chronic inflammation induced by a subseptic dose of Porphyromonas gingivalis lipopolysaccharide (LPS) exacerbated infarct expression of the proinflammatory cytokine Ccl12. Ccl12 prevented initiation of the reparative response by prolonging inflammation and inhibiting fibroblast conversion to myofibroblasts, resulting in diminished scar formation. Macrophage secretion of Ccl12 directly impaired fibronectin and collagen deposition and indirectly stimulated collagen degradation through upregulation of matrix metalloproteinase-2. In post-MI patients, circulating LPS levels strongly associated with the Ccl12 homologue monocyte chemotactic protein 1 (MCP-1). Patients with LPS levels ≥ 1 endotoxin units (EU)/ml (subseptic endotoxemia) at the time of hospitalization had increased end diastolic and systolic dimensions compared with post-MI patients with < 1 EU/ml, indicating that low yet pathological concentrations of circulating LPS adversely impact post-MI left ventricle (LV) remodeling by increasing MCP-1. Our study provides the first evidence to our knowledge that chronic inflammation inhibits reparative fibroblast activation and generates an unfavorable cardiac–healing environment through Ccl12-dependent mechanisms.

Authors

Kristine Y. DeLeon-Pennell, Rugmani Padmanabhan Iyer, Osasere K. Ero, Courtney A. Cates, Elizabeth R. Flynn, Presley L. Cannon, Mira Jung, De’Aries Shannon, Michael R. Garrett, William Buchanan, Michael E. Hall, Yonggang Ma, Merry L. Lindsey

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Figure 7

Ccr2 activation by Ccl12 induced fibroblast dysfunction and impaired wound healing.

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Ccr2 activation by Ccl12 induced fibroblast dysfunction and impaired wou...
(A) In vitro stimulation of cardiac fibroblasts with Ccl12 attenuated cell migration (by electric cell–substrate impedance sensing, ECIS) and increased cell proliferation (by BrdU uptake) independent of Ccr2. n = 5/group (5M); 4.5 ± 0.1 months for all groups. All in vitro stimulation experiments were paired. (B) Collagen I, fibronectin, TGFβ1, and α–smooth muscle actin (αSMA) significantly decreased in Ccl12-stimulated fibroblasts. Ccr2 inhibition partially restored Ccl12 effects on all ECM genes. n = 5/group (5M); 4.5 ± 0.1 months for all groups. All in vitro stimulation experiments were paired. (C) In vivo Ccl12 exposure in the post-MI LV increased cardiac rupture similar to rates observed for the LPS+MI mice. This was attenuated by administering a Ccl12 blocking antibody (Ccl12i) in vivo. (D) Administration of Ccl12i increased the 25 kDa band by 2-fold, indicating successful Ccl12 inhibition. (E) In addition, Ccl12 upregulation increased collagen turnover and (F) active MMP-2 similar to what was observed in LPS+MI mice. Ccl12i attenuated this effect. No change was observed in IgG controls. n = 4/group (2M, 2F for MI, IgG, and Ccl12i; 1M, 3F for recombinant Ccl12 [rCcl12]); MI = 4.7 ± 0.1 months; IgG = 3.6 ± 0.1 months; rCcl12 = 4.3 ± 0.2 months; Ccl12i = 3.6 ± 0.1 months. Data is shown as box and whisker plots with mean ± minimum/maximum; one-way ANOVA with Student Newman-Keuls post-test; *P < 0.05 vs. 0.1% FBS; †P < 0.05 vs. Ccl12 stimulated cells; ‡P < 0.05 vs. d7 MI.