Complement-containing small extracellular vesicles from adventitial fibroblasts induce proinflammatory and metabolic reprogramming in macrophages
Sushil Kumar, Maria G. Frid, Hui Zhang, Min Li, Suzette Riddle, R. Dale Brown, Subhash Chandra Yadav, Micaela K. Roy, Monika E. Dzieciatkowska, Angelo D’Alessandro, Kirk C. Hansen, Kurt R. Stenmark
Sushil Kumar, Maria G. Frid, Hui Zhang, Min Li, Suzette Riddle, R. Dale Brown, Subhash Chandra Yadav, Micaela K. Roy, Monika E. Dzieciatkowska, Angelo D’Alessandro, Kirk C. Hansen, Kurt R. Stenmark
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Research Article Inflammation Pulmonology

Complement-containing small extracellular vesicles from adventitial fibroblasts induce proinflammatory and metabolic reprogramming in macrophages

Abstract

Pulmonary hypertension (PH) is a severe cardiopulmonary disease characterized by complement-dependent, fibroblast-induced perivascular accumulation and proinflammatory activation of macrophages. We hypothesized that, in PH, nanoscale-sized small extracellular vesicles (sEVs), released by perivascular/adventitial fibroblasts, are critical mediators of complement-dependent proinflammatory activation of macrophages. Pulmonary adventitial fibroblasts were isolated from calves with severe PH (PH-Fibs) and age-matched controls (CO-Fibs). PH-Fibs exhibited increased secretion of sEVs, compared with CO-Fibs, and sEV biological activity was tested on mouse and bovine bone marrow–derived macrophages (BMDMs) and showed similar responses. Compared with sEVs derived from CO-Fibs, sEVs derived from PH-Fibs (PH-Fib-sEVs) induced augmented expression of proinflammatory cytokines/chemokines and metabolic genes in BMDMs. Pharmacological blockade of exosome release from PH-Fibs resulted in significant attenuation of proinflammatory activation of BMDMs. “Bottom-up” proteomic analyses revealed significant enrichment of complement and coagulation cascades in PH-Fib-sEVs, including augmented expression of the complement component C3. We therefore examined whether the PH-Fib-sEV–mediated proinflammatory activation of BMDMs was complement C3 dependent. Treatment of PH-Fibs with siC3-RNA significantly attenuated the capacity of PH-Fib-sEVs for proinflammatory activation of BMDMs. PH-Fib-sEVs mediated proglycolytic alterations and complement-dependent activation of macrophages toward a proinflammatory phenotype, as confirmed by metabolomic studies. Thus, fibroblast-released sEVs served as critical mediators of complement-induced perivascular/microenvironmental inflammation in PH.

Authors

Sushil Kumar, Maria G. Frid, Hui Zhang, Min Li, Suzette Riddle, R. Dale Brown, Subhash Chandra Yadav, Micaela K. Roy, Monika E. Dzieciatkowska, Angelo D’Alessandro, Kirk C. Hansen, Kurt R. Stenmark

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Figure 2

sEVs contribute, in large part, to promoting the proinflammatory effect of PH-Fib-CM on BMDMs.

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sEVs contribute, in large part, to promoting the proinflammatory effect o...
(A) sEVs and complete CM from PH-Fibs (n = 3) elicited increased Il6 mRNA expression in BMDMs, compared with “naive” media, whereas the effect of CM depleted of EVs (EV-free CM), or CO-Fibs complete CM or sEVs (n = 3), were not statistically significant. (B) NTA confirms that GW4869, an inhibitor of EV secretion, inhibited release of EVs by PH-Fibs into CM. (C and D) BMDMs incubated with CM from GW4869-pretreated PH-Fibs (n = 6) had significantly attenuated Il6 (C) and Il1b (D) expression, compared with BMDMs incubated with CM from untreated PH-Fibs (n = 6). Data are presented as mean ± SEM. Two-way ANOVA (A) or 1-way ANOVA (C and D) followed by Tukey’s multiple-comparison test were performed. Unpaired t test with Welch’s correction (B) was used for comparison between 2 groups. *P < 0.05, **P < 0.01, ****P < 0.0001. sEVs, small extracellular vesicles; BMDMs, bone marrow–derived macrophages; PH, pulmonary hypertension; PH-Fibs, fibroblasts of calves with severe PH; CO-Fibs, fibroblasts of age-matched controls; CM, conditioned medium; NTA, nanoparticle tracking analysis.