内含子源性27nt-microRNA对大鼠血管平滑肌细胞表型转换的影响及其机制研究OACSTPCD
Effect and mechanism of intron-derived 27-nt microRNA on phenotypic switch of rat vascular smooth muscle cells
目的 探讨内含子源性27nt-miRNA(27nt-miR)对血小板源性生长因子-BB(PDGF-BB)诱导大鼠血管平滑肌细胞(VSMCs)表型转换的影响及其分子机制.方法 用27nt-miR表达慢病毒转染培养的VSMCs,观察其对PDGF-BB诱导的VSMCs表型转换的影响;将细胞分为对照组、PDGF-BB诱导组、27nt-miR组、27nt-miR-sponge 组及27nt-miR NC 组(27nt-miR NC 组).雷帕霉素(100 nmol/L)与 MHY-1485(10 μmol/L)作用于 27nt-miR 组、27nt-miR-sponge 组及 27nt-miR NC 组,以验证 27nt-miR 是否参与mTOR与p70S6k通路的调控.用生物信息学预测27nt-miR与mTOR的靶向结合位点,用CCK-8法与EdU法分别测定VSMCs活力与增殖情况,划痕试验测定VSMCs迁移能力,实时荧光聚合酶链反应检测α-SMA、SM22α 及 OPN mRNA 表达,Western blotting 检测 α-SMA、SM22α、OPN、mTOR、p-mTOR、p70S6k 与 p-p70S6k蛋白表达.结果 CCK-8法结果示,PDGF-BB诱导组细胞增殖率较正常值高(P<0.05),27nt-miR NC组与PDGF-BB诱导组比较,差异无统计学意义(P>0.05);27nt-miR组细胞增殖率较27nt-miR NC 组低(P<0.05),27nt-miR-sponge 组与 27nt-miR NC 组比较,差异无统计学意义(P>0.05).PDGF-BB诱导组细胞迁移率较对照组高(P<0.05),27nt-miR NC组与PDGF-BB诱导组比较,差异无统计学意义(P>0.05);27nt-miR组细胞迁移率较27nt-miR NC组低(P<0.05),27nt-miR-sponge组细胞迁移率与27nt-miR NC组比较,差异无统计学意义(P>0.05).EdU法结果示,PDGF-BB诱导组细胞增殖率较对照组高(P<0.05),27nt-miR NC组与PDGF-BB诱导组细胞增殖率比较,差异无统计学意义(P>0.05);27nt-miR 组细胞增 殖率较 27nt-miR NC 组低(P<0.05),27nt-miR-sponge 组与 27nt-miR NC 组比较,差异无统计学意义(P>0.05).PDGF-BB诱导组α-SMA mRNA相对表达量较对照组低(P<0.05),两组SM22α与OPN mRNA相对表达量比较,差异无统计学意义(P>0.05).27nt-miR NC组与PDGF-BB诱导组α-SMA、SM22α、OPN mRNA相对表达量比较,差异无统计学意义(P>0.05);27nt-miR组α-SMA、SM22α mRNA相对表达量较27nt-miR NC组高(P<0.05),OPN mRNA相对表达量较27nt-miR NC组低(P<0.05);27nt-miR-sponge 组与 27nt-miR NC 组 α-SMA、SM22α mRNA 相对表达量比较,差异均无统计学意义(P>0.05),27nt-miR-sponge 组 OPN mRNA 相对表达量较 27nt-miR NC 组高(P<0.05).PDGF-BB诱导组α-SMA、SM22α蛋白相对表达量较对照组低(P<0.05);27nt-miR NC组、PDGF-BB诱导组OPN蛋白相对表达量较27nt-miR组高(P<0.05);27nt-miR组α-SMA、SM22α蛋白相对表达量较27nt-miR NC 组高(P<0.05),OPN 蛋白相对表达量较 27nt-miR NC 组低(P<0.05);27nt-miR 组 p70S6k、p-p70S6k与p-mTOR蛋白相对表达量较27nt-miR NC组低(P<0.05);各组经雷帕霉素处理后,27nt-miR-sponge组与27nt-miR NC组各蛋白相对表达量比较,差异均有统计学意义(P<0.05).27nt-miR组p70S6k、p-p70S6k、mTOR、p-mTOR 蛋白 相对表达量较 27nt-miR NC 组低(P<0.05),27nt-miR-sponge组与27nt-miR NC组p-p70S6k、mTOR、p-mTOR蛋白相对表达量比较,差异均有统计学意义(P<0.05).各组经 MHY-1485 处理后,27nt-miR 组 p70S6k、p-p70S6k、mTOR、p-mTOR 蛋白 相对表达量较 27nt-miR NC组低(P<0.05);27nt-miR-sponge组与27nt-miR NC组各蛋白相对表达量比较,差异均有统计学意义(P<0.05).结论 27nt-miR可能通过靶向mTOR/p70S6k信号通路从而调节大鼠血管平滑肌细胞增殖活力、增殖、迁移与表型转换.
Objective To investigate the effect and mechanism of intron-derived 27-nt microRNA(27nt-miR)on the phenotypic switch of rat vascular smooth muscle cells(VSMCs)induced by platelet-derived growth factor-BB(PDGF-BB).Methods VSMCs were transduced with 27nt-miR-expressing lentiviruses and their effects on phenotypic switch of VSMCs induced by PDGF-BB was observed.The cells were divided into control group,PDGF-BB induction group,27nt-miR group,27nt-miR-sponge group and 27nt-miR negative control(27nt-miR NC)group.The 27nt-miR group,27nt-miR-sponge group and 27nt-miR NC group were subjected to rapamycin(100 nmol/L)and MHY1485(10 μmol/L)to verify the involvement of 27nt-miR in the regulation of mTOR and p70S6k pathways.The target binding sites of 27nt-miRNA and mTOR were predicted by bioinformatics.The viability and proliferation of VSMCs were determined by CCK-8 and EdU cell proliferation assays.The migration ability of VSMCs was determined by the scratch assay.The relative mRNA expressions of α-SMA,SM22α and OPN were detected by qRT-PCR.The relative protein expressions of α-SMA,SM22α,OPN,mTOR,p-mTOR,p70S6k and p-p70S6k were detected by Western blotting.Results The CCK-8 assay revealed that the cell proliferation rate in the PDGF-BB induction group was higher than normal(P<0.05),while there was no difference in the cell proliferation rate between the 27nt-miR NC group and the PDGF-BB induction group(P>0.05).The cell proliferation rate in the 27nt-miR group was lower than that in the 27nt-miR NC group(P<0.05),while there was no difference in the cell proliferation rate between the 27nt-miR-sponge group and the 27nt-miR NC group(P>0.05).The cell migration rate in the 27nt-miR group was lower than that in the 27nt-miR NC group(P<0.05),while there was no difference in the cell migration rate between the 27nt-miR-sponge group and the 27nt-miR NC group(P>0.05).The EdU cell proliferation assay demonstrated that the cell proliferation rate in the PDGF-BB induction group was higher than that in the control group(P<0.05),while there was no difference in the cell proliferation rate between the 27nt-miR NC group and the PDGF-BB induction group(P>0.05).The cell proliferation rate in the 27nt-miR group was lower than that in the 27nt-miR NC group(P<0.05),while there was no difference in the cell proliferation rate between the 27nt-miR-sponge group and the 27nt-miR NC group(P>0.05).The relative mRNA expression of α-SMA in the PDGF-BB induction group was lower than that in the control group(P<0.05),whereas there was no difference in the relative mRNA expressions of SM22α and OPN between the two groups(P>0.05).The relative mRNA expressions of α-SMA,SM22α and OPN were not different between the 27nt-miR NC group and the PDGF-BB induction group(P>0.05).The relative mRNA expressions of α-SMA and SM22α in the 27nt-miR group were higher than those in the 27nt-miR NC group(P<0.05),while the relative mRNA expression of OPN in the 27nt-miR group was lower than that in the 27nt-miR NC group(P<0.05).There was no difference in the relative mRNA expressions of α-SMA and SM22α between the 27nt-miR-sponge group and the 27nt-miR NC group(P>0.05).The relative mRNA expression of OPN in the 27nt-miR-sponge group was higher than that in the 27nt-miR NC group(P<0.05).The relative protein expressions of α-SMA and SM22α in the PDGF-BB induction group were lower than those in the control group(P<0.05).The relative protein expression of OPN in the 27nt-miR NC group and the PDGF-BB induction group was higher than that in the 27nt-miR group(P<0.05).The relative protein expressions of α-SMA and SM22α in the 27nt-miR group were higher than those in the 27nt-miR NC group(P<0.05).The relative protein expression of OPN in the 27nt-miR group was lower than that in the 27nt-miR NC group(P<0.05).The relative protein expressions of p70S6k,p-p70S6k and p-mTOR in the 27nt-miR group were lower than those in the 27nt-miR NC group(P<0.05).After treatment with rapamycin,the relative expressions of all the proteins were different among the groups(P<0.05).The relative protein expressions of p70S6k,p-p70S6k,mTOR and p-mTOR in the 27nt-miR group were lower than those in the 27nt-miR NC group(P<0.05).There were differences in the relative protein expressions of p-p70S6k,mTOR and p-mTOR between the 27nt-miR-sponge group and the 27nt-miR NC group(P<0.05).After treatment with MHY-1485,the relative protein expressions of p70S6k,p-p70S6k,mTOR and p-mTOR in the 27nt-miR group were lower than those in the 27nt-miR NC group(P<0.05).The relative expressions of all the proteins were different between the 27nt-miR-sponge group and the 27nt-miR NC(P<0.05).Conclusion The 27nt-miR may regulate the viability,proliferation,migration and phenotypic switch of rat VSMCs by targeting the mTOR/p70S6k signaling pathway.
周炜潜;罗雪兰;王光耀;黄凤;欧和生
广西中医药大学附属国际壮医医院壮瑶医药研究实验室,广西 南宁 530201广西中医药大学附属国际壮医医院心血管内科,广西 南宁 530201
临床医学
27nt-microRNA血管平滑肌细胞mTOR/p70S6k信号通路表型转换
27nt-miRNAvascular smooth muscle cellsmTOR/p70S6k signaling pathwayphenotype switch
《中国现代医学杂志》 2024 (014)
36-45 / 10
国家自然科学基金(No:82060655)
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