Conclusions
FKN overexpression suppresses LPS-induced M1 type polarization of RAW264.7 cells by activating Wnt/β-catenin signaling pathway. 目的: 研究Fractalkine(CX3CL1,FKN)对脂多糖(LPS)诱导的RAW264.7巨噬细胞免疫应答的作用机制。 方法: 体外培养RAW264.7细胞,使用慢病毒技术构建过表达FKN的稳定细胞珠。细胞分为8组:(1)空白对照组;(2)LPS组,细胞给予脂多糖(1 μg/mL,12 h);(3)ICG-001组,细胞给与Wnt/β-catenin信号通路抑制剂ICG-001(10 μmol/mL,48 h);(4)过表达FKN组;(5)ICG-001+LPS组,细胞给与ICG-001(10 μmol/mL预处理36 h)后,加入脂多糖(1 μg/mL,12 h);(6)过表达FKN+LPS组,过表达FKN细胞给与脂多糖(1 μg/mL,12 h);(7)过表达FKN+ICG-001组,过表达FKN细胞给予ICG-001(10 μmol/mL,48 h);(8)过表达FKN+ICG-001+LPS组,过表达FKN细胞给与ICG-001(10 μmol/mL预处理36 h)后,加入脂多糖(1 μg/mL,12 h);应用CCK-8细胞增殖实验检测ICG-001作用于巨噬细胞中的安全浓度;应用酶联免疫吸附(ELISA)实验检测巨噬细胞上清液中M1型极化因子TNF-α和IL-6的含量;应用蛋白质免疫印记(WB)实验检测巨噬细胞中FKN、Wnt/β-catenin通路关键因子Wnt-4和β-catenin、M1型极化因子iNOS、TNF-α和IL-6的蛋白表达水平;应用免疫荧光(IF)实验检测巨噬细胞中M1型极化因子IL-6蛋白的定位。 结果: 过表达FKN的RAW264.7细胞中FKN的蛋白水平较空白对照组明显升高(P < 0.01)。CCK-8实验显示ICG- 001作用于RAW264.7细胞48 h的IC50为10 μmol/mL。与LPS组相比,ICG-001+LPS组上清液中TNF-α和IL-6的分泌量以及细胞内TNF-α、IL-6和iNOS蛋白含量均升高(P < 0.05),而细胞内FKN、Wnt-4和β-catenin蛋白含量均显著降低(P < 0.01);EXFKN+LPS组上清液中TNF-α和IL-6的分泌量以及细胞内TNF-α、IL-6和iNOS蛋白含量均显著降低(P < 0.01),而细胞内FKN、Wnt-4和β-catenin蛋白含量均显著升高(P < 0.01)。与LPS组相比,ICG-001+LPS组中IL-6在细胞质中的定位增强,而EXFKN+LPS组中IL-6在细胞质中的定位受到抑制。 结论: 过表达FKN通过激活Wnt/β-catenin信号通路抑制脂多糖诱导的巨噬细胞M1型极化。
Methods
A RAW264.7 cell model overexpressing FKN was established by transfection with the lentiviral vector CX3CL1. The effects of LPS, ICG-001 (a Wnt/β-catenin signaling pathway inhibitor), either alone or in combination, on M1 polarization of na?ve and FKN-overexpressing RAW264.7 cells were evaluated by detecting of intereukin-6 (IL-6) and tumor necrosis factor-α (TNF-α) using ELISA. The protein expressions of the inflammatory factors (iNOS, TNF-α, and IL-6), FKN, Wnt-4, and β-catenin were detected by Western blotting. The subcellular localization of IL-6 in the cells was detected by immunofluorescence assay.
Objective
To explore the mechanism by which fractalkine (CX3CL1; FKN) inhibits lipopolysaccharide (LPS)-induced immunological response in RAW264.7 cells.
Results
The RAW264.7 cell model of FKN overexpression was successfully established. In na?ve RAW264.7 cells, treatment with both ICG-001 and LPS, as compared with LPS alone, significant promoted TNF-α and IL-6 secretions, increased intracellular levels of TNF-α, IL-6 and iNOS (P < 0.05), and reduced intracellular FKN, Wnt-4 and β-catenin levels (P < 0.01). In FKN-overexpressing RAW264.7 cells, LPS treatment significantly reduced the secretion of TNF-α and IL-6 and intracellular levels of TNF-α, IL-6 and iNOS (P < 0.01), increased intracellular FKN, Wnt-4 and β-catenin protein contents (P < 0.01), and inhibited IL-6 localization in the cytoplasm; compared with LPS, the combined treatment with ICG-001 and LPS obviously enhanced IL-6 localization in the cytoplasm of the cells. Conclusions: FKN overexpression suppresses LPS-induced M1 type polarization of RAW264.7 cells by activating Wnt/β-catenin signaling pathway. 目的: 研究Fractalkine(CX3CL1,FKN)对脂多糖(LPS)诱导的RAW264.7巨噬细胞免疫应答的作用机制。 方法: 体外培养RAW264.7细胞,使用慢病毒技术构建过表达FKN的稳定细胞珠。细胞分为8组:(1)空白对照组;(2)LPS组,细胞给予脂多糖(1 μg/mL,12 h);(3)ICG-001组,细胞给与Wnt/β-catenin信号通路抑制剂ICG-001(10 μmol/mL,48 h);(4)过表达FKN组;(5)ICG-001+LPS组,细胞给与ICG-001(10 μmol/mL预处理36 h)后,加入脂多糖(1 μg/mL,12 h);(6)过表达FKN+LPS组,过表达FKN细胞给与脂多糖(1 μg/mL,12 h);(7)过表达FKN+ICG-001组,过表达FKN细胞给予ICG-001(10 μmol/mL,48 h);(8)过表达FKN+ICG-001+LPS组,过表达FKN细胞给与ICG-001(10 μmol/mL预处理36 h)后,加入脂多糖(1 μg/mL,12 h);应用CCK-8细胞增殖实验检测ICG-001作用于巨噬细胞中的安全浓度;应用酶联免疫吸附(ELISA)实验检测巨噬细胞上清液中M1型极化因子TNF-α和IL-6的含量;应用蛋白质免疫印记(WB)实验检测巨噬细胞中FKN、Wnt/β-catenin通路关键因子Wnt-4和β-catenin、M1型极化因子iNOS、TNF-α和IL-6的蛋白表达水平;应用免疫荧光(IF)实验检测巨噬细胞中M1型极化因子IL-6蛋白的定位。 结果: 过表达FKN的RAW264.7细胞中FKN的蛋白水平较空白对照组明显升高(P < 0.01)。CCK-8实验显示ICG- 001作用于RAW264.7细胞48 h的IC50为10 μmol/mL。与LPS组相比,ICG-001+LPS组上清液中TNF-α和IL-6的分泌量以及细胞内TNF-α、IL-6和iNOS蛋白含量均升高(P < 0.05),而细胞内FKN、Wnt-4和β-catenin蛋白含量均显著降低(P < 0.01);EXFKN+LPS组上清液中TNF-α和IL-6的分泌量以及细胞内TNF-α、IL-6和iNOS蛋白含量均显著降低(P < 0.01),而细胞内FKN、Wnt-4和β-catenin蛋白含量均显著升高(P < 0.01)。与LPS组相比,ICG-001+LPS组中IL-6在细胞质中的定位增强,而EXFKN+LPS组中IL-6在细胞质中的定位受到抑制。 结论: 过表达FKN通过激活Wnt/β-catenin信号通路抑制脂多糖诱导的巨噬细胞M1型极化。