机构地区:[1]河北北方学院附属第二医院肾内科,河北张家口075000
出 处:《山东医药》2023年第22期41-45,共5页Shandong Medical Journal
基 金:河北省医学科学研究课题(20210125)。
摘 要:目的探讨低分子量肝素(LMH)对糖尿病肾病(DN)足细胞损伤的影响及机制。方法将人肾小球足细胞(HGPC)分为对照(NC)组、高浓度葡萄糖(HG)组、1、5、10、15、20μmol/L LMH组,NC组细胞以含5 mmol/L葡萄糖的培养基培养;HG组细胞以含30 mmol/L的葡萄糖培养基培养;1、5、10、15、20μmol/L LMH组细胞以含30 mmol/L葡萄糖+不同浓度(1、5、10、15、20μmol/L)LMH的培养基共同培养,筛选出最佳浓度15μmol/L LMH后,又将细胞分为NC组、HG组、LMH组、BAY11-7082组、LMH+BAY11-7082组、LMH+Prostratin组。LMH组细胞以含30 mmol/L葡萄糖+15μmol/L LMH的培养基共同培养;BAY11-7082组细胞以含30 mmol/L的葡萄糖+1μmol/L BAY11-7082的培养基培养;LMH+BAY11-7082组细胞以含30 mmol/L葡萄糖+15μmol/L LMH+1μmol/L BAY11-7082的培养基培养;LMH+Prostratin组细胞以含30 mmol/L葡萄糖+15μmol/L LMH+20μmol/L Prostratin的培养基培养。采用活细胞计数法(CCK-8)检测HGPC细胞的细胞活力;Hoechst 33258染色法检测HGPC细胞的凋亡状况;Transwell小室实验检测HGPC细胞的侵袭能力;酶联免疫吸附实验检测HGPC裂解液中肿瘤坏死因子(TNF)-α、白细胞介素(IL)-6表达;蛋白免疫印迹法检测HGPC细胞中核转录因子kappa-B(NF-κB)p65、磷酸化(p)-NF-κBp65、波形蛋白(Vimentin)、纤连蛋白(FN)、神经型钙黏蛋白(N-cadherin)、上皮型钙黏蛋白(E-cadherin)表达。结果CCK-8结果显示,LMH的最适浓度为15μmol/L。药物处理24 h后,与NC组相比,HG组细胞凋亡率、侵袭细胞数升高(P均<0.05);与HG组相比,LMH组和BAY11-7082组细胞凋亡率、侵袭细胞数下降(P均<0.05);与LMH组相比,LMH+BAY11-7082组细胞凋亡率、侵袭细胞数下降(P均<0.05),LMH+Prostratin组细胞凋亡率、侵袭细胞数升高(P均<0.05)。与NC组相比,HG组TNF-α、IL-6、p-NF-κBp65、Vimentin、FN、N-cadherin蛋白表达升高,E-cadherin蛋白表达降低(P均<0.05);与HG组相比,LMH组和BAY11-7082组TNF-α、IL-6、p-NF-κBp65、VimenObjective To investigate the effect and mechanism of low-molecular-weight heparin(LMH)on podocyte injury in diabetic nephropathy(DN).Methods Human glomerular podocytes(HGPC)were divided into the control(NC)group,high glucose(HG)group,and 1,5,10,15,20μmol/L LMH group.The cells in the NC group were cultured in medium containing 5 mmol/L glucose.Cells in the HG group were cultured in medium containing 30 mmol/L glucose.Cells in 1,5,10,15,and 20μmol/L LMH groups were co-cultured with medium containing 30 mmol/L glucose+different concentrations(1,5,10,15,and 20μmol/L)of LMH.After the optimal concentration of LMH was screened,the cells were divided into the NC group,HG group,LMH group,BAY11-7082 group,LMH+BAY11-7082 group,and LMH+Prostratin group.Cells in LMH group were co-cultured with medium containing 30 mmol/L glucose and 15μmol/L LMH.Cells in BAY11-7082 group were cultured in medium containing 30 mmol/L glucose and 1μmol/L BAY11-7082.Cells in LMH+BAY11-7082 group were cultured in medium containing 30 mmol/L glucose,15μmol/L LMH and 1μmol/L BAY11-7082.Cells in LMH+Prostratin group were cultured in medium containing 30 mmol/L glucose,15μmol/L LMH,and 20μmol/L Prostratin.The viability of HGPC was detected by CCK-8.Hoechst 33258 staining was used to detect the apoptosis of HGPC.Transwell chamber assay was used to detect the invasion ability of HGPC.The expression levels of tumor necrosis factor(TNF)-αand interleukin(IL)-6 in HGPC solution of lysis were detected by enzyme linked immunosorbent assay(ELISA).Western blotting was used to detect the relative expressionlevels of nuclear transcription factor kappa-B(NF-κB)p65,phosphorylated(p)-NF-κBp65,Vimentin,Fibronectin(FN),N-cadherin and E-cadherin in HGPC.Results CCK-8 results showed that the optimal dose of LMH was 15μmol/L.Compared with the NC group,the apoptosis rate and the number of invasive cells increased in the HG group(both P<0.05).Compared with the HG group,the apoptosis rate and the number of invasive cells in LMH group and BAY11-7082 group decrea
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