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GM-CSF Expression and Macrophage Polarization in Joints of Undifferentiated Arthritis Patients Evolving to Rheumatoid Arthritis or Psoriatic Arthritis

川地163 类风湿性关节炎 医学 巨噬细胞极化 巨噬细胞集落刺激因子 关节炎 巨噬细胞 滑液 免疫学 CD90型 滑膜炎 病理 化学 细胞 骨关节炎 生物化学 CD44细胞 体外 替代医学
作者
Sara Fuentelsaz-Romero,Andrea Cuervo,Lizbeth Estrada‐Capetillo,Raquel Celis,Raquel García-Campos,Julio Ramírez,Sergi Sastre,Rafael Samaniego,Amaya Puig‐Kröger,Juan D. Cañete
出处
期刊:Frontiers in Immunology [Frontiers Media SA]
卷期号:11: 613975-613975 被引量:43
标识
DOI:10.3389/fimmu.2020.613975
摘要

Background and Aims GM-CSF-dependent macrophage polarization has been demonstrated in rheumatoid arthritis (RA). Our aim was to seek diagnostic/prognostic biomarkers for undifferentiated arthritis (UA) by analyzing GM-CSF expression and source, macrophage polarization and density in joints of patients with UA evolving to RA or PsA compared with established RA or PsA, respectively. Methods Synovial tissue (ST) from patients with UA evolving to RA (UA>RA, n=8), PsA (UA>PsA, n=9), persistent UA (UA, n=16), established RA (n=12) and PsA (n=10), and healthy controls (n=6), were analyzed. Cell source and quantitative expression of GM-CSF and proteins associated with pro-inflammatory (GM-CSF-driven) and anti-inflammatory (M-CSF-driven) macrophage polarization (activin A, TNFα, MMP12, and CD209, respectively) were assessed in ST CD163 + macrophages by multicolor immunofluorescence. GM-CSF and activin A levels were also quantified in paired synovial fluid samples. CD163 + macrophage density was determined in all groups by immunofluorescence. Results Synovial stromal cells (FAP + CD90 + fibroblast, CD90 + endothelial cells) and CD163 + sublining macrophages were the sources of GM-CSF. ST CD163 + macrophages from all groups expressed pro-inflammatory polarization markers (activin A, TNFα, and MMP12). Expression of the M-CSF-dependent anti-inflammatory marker CD209 identified two macrophage subsets (CD163 + CD209 high and CD163 + CD209 low/- ). CD209 + macrophages were more abundant in ST from healthy controls and PsA patients, although both macrophage subtypes showed similar levels of pro-inflammatory markers in all groups. In paired synovial fluid samples, activin A was detected in all patients, with higher levels in UA>RA and RA, while GM-CSF was infrequently detected. ST CD163 + macrophage density was comparable between UA>RA and UA>PsA patients, but significantly higher than in persistent UA. Conclusions GM-CSF is highly expressed by sublining CD90 + FAP + synovial fibroblasts, CD90 + activated endothelium and CD163 + macrophages in different types of arthritis. The polarization state of ST macrophages was similar in all UA and established arthritis groups, with a predominance of pro-inflammatory GM-CSF-associated markers. CD163 + macrophage density was significantly higher in the UA phases of RA and PsA compared with persistent UA. Taken together, our findings support the idea that GM-CSF is a strong driver of macrophage polarization and a potential therapeutic target not only in RA but also in PsA and all types of UA.
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