MicroRNA-584-5p/RUNX family transcription factor 2 axis mediates hypoxia-induced osteogenic differentiation of periosteal stem cells

BACKGROUND The hypoxic environment during bone healing is important in regulating the differentiation of periosteal stem cells(PSCs)into osteoblasts or chondrocytes;however,the underlying mechanisms remain unclear.AIM To determine the effect of hypoxia on PSCs,and the expression of microRNA-584-5p(miR-584-5p)and RUNX family transcription factor 2(RUNX2)in PSCs was modulated to explore the impact of the miR-584-5p/RUNX2 axis on hypoxiainduced osteogenic differentiation of PSCs.METHODS In this study,we isolated primary mouse PSCs and stimulated them with hypoxia,and the characteristics and functional genes related to PSC osteogenic differentiation were assessed.Constructs expressing miR-584-5p and RUNX2 were established to determine PSC osteogenic differentiation.RESULTS Hypoxic stimulation induced PSC osteogenic differentiation and significantly increased calcified nodules,intracellular calcium ion levels,and alkaline phosphatase(ALP)activity in PSCs.Osteogenic differentiation-related factors such as RUNX2,bone morphogenetic protein 2,hypoxia-inducible factor 1-alpha,and ALP were upregulated;in contrast,miR-584-5p was downregulated in these cells.Furthermore,upregulation of miR-584-5p significantly inhibited RUNX2 expression and hypoxia-induced PSC osteogenic differentiation.RUNX2 was the target gene of miR-584-5p,antagonizing miR-584-5p inhibition in hypoxia-induced PSC osteogenic differentiation.CONCLUSION Our study showed that the interaction of miR-584-5p and RUNX2 could mediate PSC osteogenic differentiation induced by hypoxia.

苯并[a]芘恶性转化细胞THBEc1中miR-584-5p/miR-211-5p/叉头框蛋白A1轴参与IDH1和HSPB1转录调控

目的探索苯并[a]芘(BaP)恶性转化人支气管上皮细胞T-16HBE-C1(THBEc1)中微RNA(miRNA)调控叉头框蛋白A1(FOXA1)表达上调的机制,并筛选和验证FOXA1的潜在靶基因。方法利用TargetScan,ENCORI数据库和THBEc1细胞与非转化细胞16HBE间miRNA的二代测序(NGS)结果,综合预测靶向调控FOXA1的miRNA,并通过实时荧光定量PCR(RT-qPCR)进一步筛选预测的miRNA。采用miRNA模拟物(mimics)转染THBEc1细胞,Western印迹法测定FOXA1蛋白表达水平,对靶向调控FOXA1的miRNA进行鉴定。利用hTF,JASPAR和ENCODE数据库结合FOXA1敲除细胞THBEc1-ΔFOXA1-c34和对照细胞THBEc1-ctrl间mRNA的NGS结果,综合预测FOXA1的潜在靶基因。利用RT-qPCR进一步对预测的靶基因[跨膜蛋白98(TMEM98)、IKAROS家族锌指2(IKZF2)、异柠檬酸脱氢酶1(IDH1)、肿瘤坏死因子受体相关因子5(TRAF5)、骨形态发生蛋白2型受体(BMPR2)、热休克蛋白B1(HSPB1)、Runt相关转录因子2(RUNX2)、golgin A7家族成员B(GOLGA7B)和维甲酸相关孤核受体A(RORA)]进行筛选。通过转染过表达质粒构建稳定表达FOXA1的细胞模型THBEc1-ΔFOXA1-c34-oe,即FOXA1功能回补,并利用RT-qPCR和Western印迹法验证FOXA1的潜在靶基因。结果TargetScan和ENCORI数据库分别预测到213和145个可能靶向调控FOXA1的miRNA。NGS共发现351个miRNA在THBEc1细胞中表达下调(差异倍数<0.5,且错误发现率<0.05),其中hsa-miR-584-5p(miR-584-5p),hsa-miR-142-5p(miR-142-5p)和hsa-miR-211-5p(miR-211-5p)在上述2个数据库中均被预测可靶向调控FOXA1。RT-qPCR结果证实,THBEc1细胞中miR-584-5p,miR-142-5p和miR-211-5p表达水平显著低于16HBE细胞(P<0.01)。转染miR-584-5p模拟物或miR-211-5p模拟物均可显著下调THBEc1细胞FOXA1蛋白表达水平(P<0.01),而转染miR-142-5p模拟物对THBEc1细胞FOXA1蛋白表达水平无明显影响。THBEc1-ΔFOXA1-c34和THBEc1-ctrl细胞间的20个差异表达基因(差异倍数<0.5或>2,且错误发现率<0.05)被hTF,JASPAR和ENCODE数据库均预测为FOXA1的潜在靶基因。RT-qPCR结果显示,在THBEc1-ΔFOXA1-c34中,TMEM98,IKZF2,IDH1,TRAF5,BMPR2,HSPB1和RUNX2 mRNA表达水平显著下调(P<0.05,P<0.01),GOLGA7B和RORA mRNA表达水平显著上调(P<0.05,P<0.01);在THBEc1-ΔFOXA1-c34-oe中,IDH1和HSPB1的mRNA表达水平显著上调(P<0.01),余7个基因mRNA表达水平未见改变。Western印迹结果显示,THBEc1-ΔFOXA1-c34细胞中IDH1和HSPB1表达水平较THBEc1-ctrl均显著下调(P<0.01);而恢复FOXA1表达的THBEc1-ΔFOXA1-c34-oe细胞中IDH1和HSPB1表达水平较对照细胞THBEc1-ΔFOXA1-c34-ctrl均显著上调(P<0.01)。结论BaP恶性转化细胞THBEc1中miR-584-5p/miR-211-5p/FOXA1轴参与IDH1和HSPB1转录调控。

大豆皂苷调控miR-584-5p/HDAC1通路对子宫内膜癌细胞增殖及凋亡的影响

目的研究大豆皂苷调控微小RNA-584-5p(microRNA-584-5p,miR-584-5p)/组蛋白去乙酰化酶1(histone deacetylasel,HDAC1)通路对子宫内膜癌(endometrial cancer,EC)细胞增殖及凋亡的影响。方法以终浓度Oltg/rml、20μg/ml、40μg/ml、80μg/ml、120μg/ml、160μg/ml的大豆皂苷处理体外培养的人EC细胞系HEC-1-A,以细胞计数试剂盒8(cell counting Kit-8,CCK-8)法测定各浓度处理后的细胞活力,计算半数抑制浓度(half maximal inhibitory concentration,IC_(50))。将对数生长期的HEC-1-A细胞随机分为对照组、大豆皂苷组、miR-584-5p抑制剂组、大豆皂苷+miR-584-5p抑制剂组、大豆皂苷+miR-584-5p抑制剂阴性对照组,分组转染及用药处理后,以CCK-8法测定各组细胞活力;以流式细胞实验检测各组细胞凋亡率;以免疫印迹实验检测各组细胞HDAC1蛋白、增殖相关蛋白增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)及凋亡相关蛋白[天冬氨酸特异性半胱氨酸蛋白酶9(cysteine-containing aspartate-specific proteases 9,caspase-9)、B淋巴细胞瘤-2相关X蛋白(B-cell lymphoma-2-associated X protein,Bax)]表达;以实时荧光定量PCR(real-time quantitative PCR,qRT-PCR)实验检测各组细胞miR-584-5p与HDAC1 mRNA表达。结果不同浓度大豆皂苷可抑制HEC-1-A细胞生长,IC_(50)为98.56μg/ml。与对照组相比,大豆皂苷组与大豆皂苷+miR-584-5p抑制剂阴性对照组的细胞活力、PCNA蛋白表达、HDACl mRNA及蛋白表达降低(P<0.05),凋亡率、caspase-9及Bax蛋白表达、miR-584-5p表达增高(P<0.05);miR-584-5p抑制剂组的细胞各指标与大豆皂苷组相反。miR-584-5p抑制剂可减弱大豆皂苷对细胞各指标的作用。结论大豆皂苷可上调miR-584-5p表达,下调HDAC1表达,促使EC细胞凋亡,抑制其增殖。

miR-584-5p对鼻咽癌远处转移及临床预后的预测作用

目的研究miR-584-5p在鼻咽癌远处转移中的作用,探讨miR-584-5p作为临床预后预测指标的可能性。方法收集有远处转移(转移组,n=26)和仅有原发病灶(非转移组,n=32)鼻咽癌活检标本共58例。用实时荧光定量RT-PCR方法检测鼻咽癌组织miR-584-5p的表达水平,分析miR-584-5p与临床病理特征及预后的关系。结果与非转移组比较,转移组miR-584-5p表达显著上调(χ~2=5. 486,P <0. 05)。miR-584-5p表达水平与性别、年龄、发病部位、T分期、临床分期及颈部淋巴结转移均无明显相关性(P>0. 05)。以miR-584-5p相对表达量中位值2^(-ΔΔCt)=1. 76为截断值,Kaplan-Meier生存曲线和Logrank检验结果显示,高表达组鼻咽癌患者无进展生存时间及5年总生存率与低表达组比较,差异均有统计学意义(χ~2=5. 486,P <0. 05;χ~2=4. 542,P <0. 05)。单因素Cox比例风险回归分析结果显示,miR-584-5p高表达组鼻咽癌患者死亡风险高于低表达组(RR=1. 09,P <0. 05)。结论 miR-584-5p表达上调可促进鼻咽癌远处转移,与临床预后呈负相关。

lncRNA NEAT1调控miR-22-3p促进NHE5的表达对神经胶质瘤细胞迁移和侵袭的影响

目的探讨lncRNA NEAT1对神经胶质瘤细胞迁移和侵袭的影响及相关机制。方法运用qRT-PCR检测神经胶质瘤细胞系C6中lncRNA NEAT1、miR-22-3p、NHE5的mRNA相对表达量;蛋白质免疫印迹检测NHE5的蛋白质表达;运用细胞集落形成实验、划痕实验和Transwell实验检测细胞的增殖、迁移和侵袭情况。结果在神经胶质瘤细胞系C6中lncRNA NEAT1表达升高,miR-22-3p表达降低;过表达miR-22-3p可抑制神经胶质瘤细胞系C6的迁移和侵袭;miR-22-3p可降低NHE5的表达,NHE5可促进神经胶质瘤细胞迁移和侵袭。lncRNA NEAT1可负向调控miR-22-3p的表达,促进C6细胞的迁移和侵袭。结论lncRNA NEAT1通过负向调控miR-22-3p促进NHE5的表达促进神经胶质瘤细胞的迁移和侵袭。

沉默lncRNA SLC16A1-AS1对脑胶质瘤细胞恶性生物学行为的影响

目的探讨沉默长链非编码RNA(lncRNA)SLC16A1-AS1对脑胶质瘤细胞恶性生物学行为的影响。方法PCR检测2021年5月至2023年1月手术切除的62例脑胶质瘤组织lncRNA SLC16A1-AS1、微小RNA(miR)-584-5p以细胞外蛋白调节激酶1(MAPK1)m RNA,免疫印迹法检测MAPK1蛋白表达;以瘤旁组织(距离肿瘤边缘>2 cm)作为正常脑组织。从胶质瘤组织中分离、培养胶质瘤细胞,进行CD133、Neatin免疫荧光染色鉴定;转染不同质粒沉默lncRNA SLC16A1-AS1、上调或下调miR-584-5p表达;应用CCK-8法、划痕实验、Transwell实验和流式细胞术检测细胞增殖、迁移、侵袭和凋亡情况;免疫印迹法检测细胞MAPK1、细胞周期素D1(CyclinD1)、基质金属蛋白酶(MMP)-2、caspase-3蛋白表达;双荧光素酶报告基因实验验证lncRNA SLC16A1-AS1、miR-584-5p和MAPK1的靶向关系。结果胶质瘤组织lncRNA SLC16A1-AS1、MAPK1呈高表达(P<0.05),miR-584-5p呈低表达(P<0.05)。免疫荧光染色显示,分离培养的细胞CD133、Nestin均呈阳性表达。沉默lncRNA SLC16A1-AS1表达,明显抑制体外培养的胶质瘤细胞增殖、迁移、侵袭(P<0.05),促进细胞凋亡(P<0.05),明显下调细胞CyclinD1、MMP-2、MMP-9蛋白表达(P<0.05),明显上调miR-584-5p、caspase-3表达。抑制miR-584-5p明显逆转沉默lncRNA SLC16A1-AS1对体外培养的价胶质瘤细胞的作用。双荧光素酶报告基因实验证实lncRNA SLC16A1-AS1与miR-584-5p/MAPK1存在靶向调节关系。结论胶质瘤组织lncRNA SLC16A1-AS1呈高表达,沉默lncRNA SLC16A1-AS1可以上调miR-584-5p表达,抑制MAPK1表达,进而抑制胶质瘤细胞的增殖、迁移、侵袭,促进细胞凋亡。

miR-584-5p通过下调MMP-14抑制乳腺癌细胞生物学行为

目的探讨微小RNA-584-5p(miR-584-5p)对乳腺癌细胞生物学行为(增殖、迁移和侵袭)的影响及其作用机制。方法选择人正常乳腺上皮细胞MCF10A及乳腺癌细胞MDA-MB-231、SK-BR-3和MCF-7;取对数生长期的MCF-7细胞,应用LipofectamineTM 2000转染试剂盒对其进行转染,并分为7组:空白组(未转染的MCF-7细胞)、模拟物-阴性对照组(mimic-negative control,mimic-NC,mimic-NC组;转染mimic-NC)、miR-584-5p mimic组(转染miR-584-5p mimic)、pcDNA组[转染过表达基质金属蛋白酶-14(MMP-14)的pcDNA3.1质粒阴性对照(pcDNA3.1)]、MMP-14组[转染过表达MMP-14的pcDNA3.1质粒(pcDNA3.1-MMP-14)]、mimic-NC+MMP-14组(共转染mimic-NC和pcDNA3.1-MMP-14)及miR-584-5p mimic+MMP-14组(共转染miR-584-5p mimic和pcDNA3.1-MMP-14)。荧光定量PCR法检测MCF10A、MDA-MB-231、SK-BR-3和MCF-7细胞中的miR-584-5p表达水平以及各组MCF-7细胞中miR-584-5p及MMP-14 mRNA表达水平;蛋白印迹法检测各组MCF-7细胞中MMP-14蛋白表达;采用细胞计数试剂盒-8(CCK-8)、划痕实验和Transwell实验分别检测各组MCF-7细胞的增殖、迁移及侵袭情况;采用双荧光素酶报告基因实验检测miR-584-5p与MMP-14的靶向关系。结果与人正常乳腺上皮细胞MCF10A比较,乳腺癌MDA-MB-231、SK-BR-3和MCF-7细胞中miR-584-5p表达水平均降低(P<0.05),且MCF-7细胞中miR-584-5p表达水平最低。与空白组和mimic-NC组比较,miR-584-5p mimic组MCF-7细胞的miR-584-5p表达水平升高,MMP-14 mRNA和蛋白表达水平、增殖活力、划痕愈合率和侵袭细胞数降低或减少(P<0.05);与空白组和pcDNA组比较,MMP-14组MCF-7细胞的MMP-14 mRNA和蛋白表达水平、增殖活力、划痕愈合率及侵袭细胞数增高或增多(P<0.05);与MMP-14组及mimic-NC+MMP-14组比较,miR-584-5p mimic+MMP-14组MCF-7细胞的miR-584-5p表达水平升高,MMP-14 mRNA和蛋白表达水平、增殖活力、划痕愈合率和侵袭细胞数降低或减少(P<0.05);miR-584-5p mimic+MMP-14组MCF-7细胞的MMP-14 mRNA和蛋白表达水平、增殖活力、划痕愈合率及侵袭细胞数高于或多于miR-584-5p mimic组(P<0.05)。双荧光素酶报告基因实验检测结果显示miR-584-5p可靶向作用于MMP-14启动子区。结论miR-584-5p可靶向调控MMP-14的表达;过表达miR-584-5p通过下调MMP-14抑制乳腺癌细胞的增殖、迁移和侵袭。