百令胶囊上调miR-145-5p逆转TGF-β_(1)/Smad3通路机制初探

目的探讨百令胶囊(BLC)对慢性阻塞性肺疾病(COPD)模型大鼠肺损伤的改善作用,以及对香烟烟雾提取物(CSE)作用下人支气管上皮细胞BEAS-2B生长的影响。方法将60只SD大鼠随机分为正常对照组(A组,灌胃生理盐水2 mL),模型组(B组,灌胃生理盐水2 mL),BLC组(C组,灌胃BLC 5.5 mg/kg),miR-145-5p inhibitorNC组(D组,灌胃BLC 5.5 mg/kg+尾静脉注射miR-145-5p inhibitorNC 6μL),miR-145-5p inhibitor组(E组,灌胃BLC 5.5 mg/kg+尾静脉注射miR-145-5p inhibitor 6μL),各12只。以香烟烟雾吸入法复制大鼠COPD模型。建模成功后灌胃相应药物或生理盐水(每日1次),尾静脉注射相应药物(每周1次),连续8周。以0(空白对照),3%,5%,10%,20%CSE,以及加5%,10%,20%,40%的BLC药物血清(BLC-S)孵育细胞48 h。检测大鼠潮气量(TV)、呼气峰流量(PEF)、分钟通气量(MV)、用力肺活量(FVC)和第0.3秒用力呼气容积(FEV_(0.3));观察肺组织病理形态;免疫组化法检测Smad3表达水平,用酶联免疫吸附试验(ELISA)法测定转化生长因子(TGF)-β_(1)表达水平,采用实时荧光定量聚合酶链反应(RT-qPCR)法检测miR-145-5p mRNA表达水平。采用CCK-8法检测细胞活力。结果与B组比较,C组及D组大鼠TV,PEF,MV,FVC,FEV0.3均显著升高;与D组比较,E组大鼠上述指标均显著降低(P<0.05)。与B组比较,C组及D组大鼠肺组织病理形态显著改善,平均肺泡数显著增加,肺泡直径显著减小;与D组比较,E组大鼠肺组织病理形态未改善,且平均肺泡数显著减少,肺泡直径显著增长(P<0.05)。与5%CSE条件比较,5%CSE+20%BLC-S条件下的细胞活力显著增强(P<0.05)。与B组比较,C组及D组大鼠肺组织中Smad3,TGF-β_(1)的表达水平均显著降低,miR-145-5p mRNA表达水平显著升高(P<0.05);与D组比较,E组大鼠肺组织中Smad3,TGF-β_(1)的表达水平均显著升高,miR-145-5p mRNA表达水平显著降低(P<0.05)。与5%CSE条件比较,5%CSE+20%BLC-S条件下细胞Smad3和TGF-β_(1)的表达水平均显著降低,miR-145-5p mRNA表达水平显著升高(P<0.05);与5%CSE+20%BLC-S+inhibitor NC条件比较,同水平inhibitor条件下细胞Smad3及TGF-β_(1)表达水平均显著升高(P<0.05)。结论BLC在体内和体外均显示出对香烟诱导COPD的保护作用,其机制可能与上调miR-145-5p水平逆转香烟暴露激活的TGF-β_(1)/Smad3信号通路有关。

Experimental study of TGF-β1/Smads pathway inhibition of macrophage polarization based on miR145-5P negative feedback regulation

imbalance of synovial macrophages in patients with rheumatoid arthritis(RA).Methods:Human mononuclear cells(THP‑1)at logarithmic growth stage were induced into M1‑type macrophages,and RA synovial fibroblasts M1‑type macrophages were co‑cultured into synovial macrophages.Synovial macrophages were divided into four groups:RA group(blank group),TGF‑β1 group(model group)and miR145‑5P overexpression group(TGF‑β1+miR145‑5P mimics group)and miR145‑5P overexpression negative control group(TGF‑β1+miR145‑5P‑mimics‑NC group).The blank group did not receive any treatment,and the other three groups were induced by TGF‑β1 in the medium for 48 h.Transfection miR145‑5p mimic and miR145‑5P‑mimics‑NC were added to co‑culture medium,and IL‑6,IL‑6 and IL‑6 of synovial macrophages were detected by ELISA.CD163 expression.Rt‑qpcr was used to detect miR145‑5p mRNA,TGF‑β1mRNA,Smad3mRNA,Smad7mRNA expression level.The expression of TGF‑β1/Smads pathway related proteins was detected by Western Blotting.Results:Compared with blank group,IL‑6 level was up‑regulated(P<0.01),and CD163 level was down‑regulated in model group(P<0.05),suggesting that TGF‑β1 could induce intensified immune inflammatory response.Compared with the negative miR145‑5P overexpression control group and model group,The expression of miR145‑5P overexpression group molecule CD163 was significantly increased by ELISA(P<0.01),and the expression of inflammatory factor IL‑6 was decreased(P<0.05).PCR showed that miR145‑5P mRNA expression level was significantly increased in miR145‑5P overexpression group,Smad3 mRNA and TGF‑β1 mRNA were significantly decreased,and Smad7 mRNA was significantly increased(P<0.01).WB method showed that the anti‑inflammatory protein Smad7 was significantly increased,while TGF‑β1 and Smad3 were significantly decreased(P<0.01).Transwell chamber results confirmed that miR145‑5P overexpression group significantly reduced macrophage invasion(P<0.01).Correlation analysis showed that miR145‑5P was negatively correlated with Smad3 and positively correlated with Smad7(P<0.01).Conclusion:miR145‑5P may inhibit macrophage polarization in RA patients by targeting Smad3 protein,negatively regulating TGF‑β1/Smads pathway,and alleviating immune inflammation.

佐剂性关节炎大鼠miR145-5p/Smads通路变化、巨噬细胞极化及其相关性分析

目的:探究佐剂性关节炎大鼠miR145-5p/Smads通路变化与巨噬细胞极化之间的联系。方法:12只大鼠使用随机数字表法分成正常组和注射弗氏完全佐剂(0.1 mL/只)致炎的模型组,6只/组。大鼠关节炎形成后第12天,酶联免疫吸附试验检测滑膜组织中巨噬细胞极化标志物IL-8、CD206表达。免疫蛋白印记法检测滑膜组织中TGF-β1/Smads通路因子表达。RT-qPCR法检测滑膜组织中miR145-5p、Smads3、Smads7的表达。结果:与正常组相比,模型组大鼠IL-8、TGF-β1、Smad3的表达水平明显升高(P<0.05);CD206、Smad7、miR145-5p的表达水平显著降低(P<0.01)。相关性结果显示,IL-8与Smad3呈正相关(P<0.01),Smad7呈负相关(P<0.05);CD206与Smad3呈负相关(P<0.01),与Smad7呈正相关(P<0.05);miR145-5p与Smad3呈负相关(P<0.01),与Smad7呈正相关(P<0.01)。结论:miR145-5p可能通过抑制Smad3表达,进而抑制TGF-β1/Smads通路过激活,调节巨噬细胞极化,抑制佐剂性关节炎的发展。

Correlation analysis of changes in miR145‑5p/Smads pathway and macrophage polarization in adjuvant arthritis rats

Objective:To explore the relationship between the changes of miR145‑5p/Smads pathway and macrophage polarization in adjuvant arthritis rats.Methods:Twelve rats were divided into normal group and model group induced by freund's complete adjuvant(0.1 mL/mouse)by random number table method,with 6 rats in each group.The expression of inflammatory polarization markers IL‑8 and CD206 in synovial tissue was detected by enzyme‑linked immunosorbent assay on the 12th day after the formation of arthritis in rats.Western blotting was used to detect the expression of TGF‑β1/Smads pathway factors in synovial tissues.The expression of miR145‑5P,Smads3 and Smads7 in synovial tissue was detected by RT‑qPCR.Results:Compared with normal group,the expression levels of IL‑8,TGF‑β1 and Smad3 in model group were significantly increased(P<0.05);The expression levels of CD206,Smad7 and miR145‑5P were significantly decreased(P<0.01).The correlation results showed that IL‑8 was positively correlated with Smad3(P<0.01),IL‑8 was negatively correlated with Smad7(P<0.05),CD206 was negatively correlated with Smad3(P<0.01)and positively correlated with Smad7(P<0.05).miR145‑5p was negatively correlated with Smad3(P<0.01)and positively correlated with Smad7(P<0.01).Conclusion:miR145‑5p may inhibit the overactivation of TGF‑β1/Smads pathway,regulate macrophage polarization,and inhibit the development of adjuvant arthritis by inhibiting Smad3 expression.

基于miR145⁃5p负反馈调控TGF⁃β1/Smads通路抑制巨噬细胞极化的实验研究

目的:探讨miR145‐5p过表达对类风湿性关节炎(RA)患者滑膜巨噬细胞极化失衡的影响。方法:取对数生长期的人单核细胞(THP‐1)诱导为成M1型巨噬细胞,将RA滑膜成纤维细胞M1型巨噬细胞与共培养成滑膜巨噬细胞。滑膜巨噬细胞分为4组:RA组(空白组)、TGF‐β1组(模型组)、miR145‐5p过表达组(TGF‐β1+miR145‐5p mimics组)、miR145‐5p过表达阴性对照组(TGF‐β1+miR145‐5p‐mimics‐NC组)。空白组不做任何处理,其余3组均在培养基中TGF‐β1处理诱导48 h。转染miR145‐5p‐mimic和miR145‐5p‐mimics‐NC至共培养基中,ELISA法检测滑膜巨噬细胞IL‐6、CD163表达。RT‐qPCR检测miRNA145‐5p、TGF‐β1mRNA、Smad3mRNA、Smad7mRNA表达水平。WB免疫印迹法检测TGF‐β1/Smads通路相关蛋白表达。结果:与空白组比较,模型组IL‐6水平上调(P<0.01),CD163水平下调(P<0.05),提示TGF‐β1可诱导加剧免疫炎症反应;与miR145‐5p过表达阴性对照组、模型组相比,ELISA法显示miR145‐5p过表达组抑炎分子CD163明显升高(P<0.01),致炎因子IL‐6表达降低(P<0.05);PCR显示miR145‐5p过表达组miR145‐5p mRNA表达水平明显升高,Smad3 mRNA、TGF‐β1 mRNA明显降低,Smad7 mRNA明显升高(P<0.01);WB法显示miR145‐5p过表达组抑炎蛋白Smad7明显升高,TGF‐β1、Smad3蛋白明显降低(P<0.01);transwell小室结果证实miR145‐5p过表达组显著减少巨噬细胞侵袭(P<0.01);相关性分析显示miR145‐5p与Smad3负相关,与Smad7呈正相关(P<0.01)。结论:miR145‐5p可能通过靶向抑制Smad3蛋白,负反馈调控TGF‐β1/Smads通路,抑制RA患者巨噬细胞极化,缓解免疫炎症反应。