Department of Oral Biology, University Clinics for Dentistry, Medical University of Vienna, Sensengasse 2a, 1090 Vienna, Austria.
Laboratory for Cardiac and Thoracic Diagnosis, Regeneration and Applied Immunology, Währingergürtel 18-20, 1090 Vienna, Austria.
Int J Mol Sci. 2020 Nov 13;21(22):8569. doi: 10.3390/ijms21228569.
Osteoclastogenesis required for bone remodeling is also a key pathologic mechanism of inflammatory osteolysis being controlled by paracrine factors released from dying cells. The secretome of irradiated, dying peripheral blood mononuclear cells (PBMCs) has a major impact on the differentiation of myeloid cells into dendritic cells, and macrophage polarization. The impact on osteoclastogenesis, however, has not been reported. For this aim, we used murine bone marrow macrophages exposed to RANKL and M-CSF to initiate osteoclastogenesis, with and without the secretome obtained from γ-irradiated PBMCs. We reported that the secretome significantly enhanced in vitro osteoclastogenesis as determined by means of histochemical staining of the tartrate-resistant acid phosphatase (TRAP), as well as the expression of the respective target genes, including TRAP and cathepsin K. Considering that TGF-β enhanced osteoclastogenesis, we confirmed the TGF-β activity in the secretome with a bioassay that was based on the increased expression of IL11 in fibroblasts. Neutralizing TGF-β by an antibody decreased the ability of the secretome to support osteoclastogenesis. These findings suggested that TGF-β released by irradiated PBMCs could enhance the process of osteoclastogenesis in vitro.
破骨细胞生成是骨重建所必需的,也是炎症性骨溶解的关键病理机制,后者受死亡细胞分泌的旁分泌因子所控制。辐照后死亡的外周血单个核细胞 (PBMC) 的分泌组对髓样细胞向树突状细胞和巨噬细胞极化的分化有重大影响。然而,其对破骨细胞生成的影响尚未有报道。为此,我们使用骨髓巨噬细胞,在 RANKL 和 M-CSF 的作用下启动破骨细胞生成,同时使用来自γ辐照 PBMC 的分泌组。我们报告称,分泌组通过抗酒石酸酸性磷酸酶(TRAP)的组织化学染色以及相应靶基因(包括 TRAP 和组织蛋白酶 K)的表达,显著增强了体外破骨细胞生成。考虑到 TGF-β 增强了破骨细胞生成,我们通过基于成纤维细胞中 IL11 表达增加的生物测定法,证实了分泌组中的 TGF-β 活性。通过抗体中和 TGF-β 降低了分泌组支持破骨细胞生成的能力。这些发现表明,辐照 PBMC 释放的 TGF-β 可以增强体外破骨细胞生成过程。
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