CircR-ZC3HC1 mediates MiR-384-5p/SIRT1 axis to promote neuronal autophagy and relieves ischemic stroke

Objective:Circular RNAs(circRNAs)have been shown to involve in pathological processes of ischemic stroke(IS),including autophagy.This study was designed to explore the effect of circR-ZC3HC1 on neuronal autophagy in IS and the related mechanisms.Methods:Expression of circR-ZC3HC1 in blood samples of IS patients and healthy controls was detected.Hippocampal neurons were treated with oxygen and glucose deprivation(OGD)to establish IS in vitro model.The expression of LC3 and p62 and the number of autophagosomes were examined to evaluate the autophagy level of OGD induced neurons using western blotting and transmission electron microscope.Cell apoptosis rate and the expression of cleaved caspase-3,Bax,and Bcl-2 were assessed byflow cytometry and western blotting.The binding relationships among circR-ZC3HC1,miR-384-5p,and SIRT1 were predicted and verified.Results:Low expression of circR-ZC3HC1 was found in blood samples of IS patients and OGD-treated neurons.Overexpressed circR-ZC3HC1 or inhibited miR-384-5p expression promoted autophagy and inhibited apoptosis of OGD-treated neurons,which could be reversed by further 3-MA treatment.Mechanistically,circR-ZC3HC1 targeted miR-384-5p to mediate SIRT1 expression.miR-384-5p overexpression or SIRT1 knockdown in the presence of circR-ZC3HC1 overexpression in OGD-treated neurons lead to reduced autophagy and enhanced apoptosis.Conclusion:Collectively,circR-ZC3HC1 promoted neuronal autophagy to attenuate IS via miR-384-5p/SIRT1 axis.

LncRNA SNHG14调控miR-656-3p/SIRT5通路加重肝癌侵袭和迁移

目的:探讨长链非编码RNA(lncRNA)小核仁RNA宿主基因14(SNHG14)对肝细胞癌(HCC)细胞侵袭和迁移的影响及机制。方法:采用实时荧光定量聚合酶链式反应(qRT-PCR)检测肝癌细胞SNHG14和miR-656-3p的表达。与sh-SNHG14,miR-656-3p抑制剂,miR-656-3p模拟物,pcDNA3.1-SIRT5共转染后,检测HepG2和MHCC97H细胞增殖、侵袭和迁移。然后用qRT-PCR测定SNHG14、miR-656-3p和SIRT5的表达水平,荧光素酶报告基因检测和RNA下调SNHG14与miR-656-3p之间的关系,以及miR-656-3p与SIRT5之间的关系。结果:HCC细胞中SNHG14表达上调,miR-656-3p表达下调。抑制SNHG14和miR-656-3p过表达,可抑制HepG2和MHCC97H细胞增殖,侵袭和迁移。SNHG14直接作用于miR-656-3p,SIRT5是miR-656-3p的靶基因。miR-656-3p抑制剂或pcDNA3.1-SIRT5可逆转sh-SN HG14对肝癌细胞增殖、侵袭和迁移的抑制作用。结论:SNHG14通过调节miR-656-3p/SIRT5轴促进肝癌细胞的侵袭和迁移。

模拟失重下miR-138-5p靶向SIRT1负调控成骨细胞分化的研究

背景机械刺激对于维持骨骼重塑和平衡至关重要,机械卸载引起的骨骼系统损伤是长期航天飞行的主要局限性之一。研究表明微小RNA(miRNA)可通过调控与骨形成相关的基因和信号通路调节成骨细胞功能。目的探究模拟失重下mi R-138-5p/SIRT1信号通路对成骨细胞分化的影响,为失重性骨质丢失的在体靶向干预寻求治疗靶点。方法利用2D回转器对前成骨细胞MC3T3-E1进行模拟失重处理,验证沉默信息调节因子2相关酶I(SIRT1)及miR-138-5p在模拟失重下的表达发生变化;向MC3T3-E1细胞中转染miR-138-5p mimic、inhibitor、pcDNA3.1(+)-SIRT1及相应的阴性对照进行功能验证;向MC3T3-E1细胞中转染inhibitor-NC、miR-138-5p inhibitor后模拟失重处理48 h进行挽救实验;采用qRT-PCR方法检测mi RNA及SIRT1、Runx2、Osx的mRNA表达变化;采用Western blot方法检测SIRT1、Runx2、Osx的蛋白表达变化;采用碱性磷酸酶(alkaline phosphatase,ALP)活性检测和ALP染色方法检测成骨细胞分化能力的变化。结果模拟失重下,MC3T3-E1细胞中Runx2、SIRT1的mRNA及蛋白均表达下降(P<0.01或P<0.05);转染miR-138-5p mimic和inhibitor后,qRT-PCR、Western blot、ALP活性及ALP染色检测均表明过表达miR-138-5p能够显著抑制成骨细胞分化,而抑制miR-138-5p能够促进MC3T3-E1细胞分化(P<0.05或P<0.01)。miR-138-5p mimic与pEX-SIRT1共转染实验表明miR-138-5p通过抑制SIRT1负调控成骨细胞分化(P<0.01)。此外,抑制miR-138-5p可以降低模拟失重对成骨细胞的分化抑制,表现为促进SIRT1、Runx2、Osx mRNA和蛋白表达(P<0.01)。结论 SIRT1表达在模拟失重下下调,而miR-138-5p表达上调;miR-138-5p通过直接靶向SIRT1调控Runx2、Osx的mRNA及蛋白表达,抑制成骨细胞分化;此外,抑制miR-138-5p/SIRT1通路可以部分降低模拟失重对成骨细胞的分化抑制,miR-138-5p可以作为潜在的干预靶点。

CircPTPN22作为miR-766-3p分子海绵促进类风湿关节炎病理进程

目的本研究旨在探索circPTPN22在类风湿关节炎(RA)外周血单个核细胞(PBMCs)中的表达及参与RA的机制。方法RT-PCR检测circPTPN22在20例RA和20例健康人(HCs)PBMCs中的表达,生物信息学预测能与其结合的microRNA(miRNA),并用功能学实验和双荧光素酶试验进行验证。检测miRNA在RA患者PBMCs中的表达并计算受试者工作特征曲线(ROC)评估miRNA在RA中的临床意义。结果CircPTPN22表达水平在RA PBMCs中显著降低。ROC分析提示circPTPN22是RA患者的潜在诊断生物标志物(AUC=0.7025),相关性分析结果显示cirPTPN22的表达与RA的SJC、anti-CCP呈负相关关系(SJC:r=-0.723;anti-CCP:r=-0.618)。MiR-766-3p在RA PBMCs中显著上调;ROC分析提示miR-766-3p的表达可以将RA患者与HCs区分开来(AUC=0.9125)。生物信息学分析、双荧光素酶试验和功能学实验显示circPTPN22能抑制miR-766-3p的表达,miR-766-3p通过调控下游靶基因SIRT5参与RA。结论CircPTPN22通过与miR-766-3p竞争性结合调控下游靶基因SIRT5参与RA的发生与发展,且circPTPN22是RA的潜在诊断生物标志物。