Long Non-coding RNA MEG3 Induces Renal Cell Carcinoma Cells Apoptosis by Activating the Mitochondrial Pathway

Summary： This study aimed to examine the effect of long non-coding RNA （LncRNA） MEG3 on the biological behaviors of renal cell carcinoma （RCC） cells 786-0 and the possible mechanism. MEG3 expression levels were detected by RT-qPCR in Rmaor tissues and adjacent non-tumor tissues from 29 RCC patients and in RCC lines 786-0 and SN12 and human embryonic kidney cell line 293T. Plasmids GV144-MEG3 （MEG3 overexpression plasmid） and GV144 （control plasmid） were stably transfected into 786-0 cells by using lipofectamine 2000. Cell viabilities were determined by MTT, cell apoptosis rates by flow cytometry following PE Annexin V and 7AAD staining, apoptosis-related protein expressions by Western blotting, and Bcl-2 mRNA by RT-qPCR in the transfected cells. The results showed that MEG3 was evidently downregulated in RCC tissues （P〈0.05） and RCC cell lines （P〈0.05）. The viabilities of 786-0 cells were decreased significantly after transfection with GV144-MEG3 for over 24 h （P〈0.05）. Consistently, the apoptosis rate was significantly increased in 786-0 cells transfected with GV144-MEG3 for 48 h （P〈0.05）. Furthermore, overexpression of MEG3 could reduce the expression of Bcl-2 and procaspase-9 proteins, enhance the expression of cleaved caspase-9 protein, and promote the release of cytochrome c protein to cytoplasm （P〈0.05）. Additionally, Bcl-2 mRNA level was declined by MEG3 overexpression （P〈0.05）. It was concluded that MEG3 induces the apoptosis of RCC cells possibly by activating the mitochondrial pathway.

Decreased expression of the long non-coding RNA HOXD-AS2 promotes gastric cancer progression by targeting HOXD8 and activating PI3K/Akt signaling pathway

BACKGROUND Long non-coding RNAs(lncRNAs) have been shown to be associated with many tumors. However, the specific mechanism of lncRNAs in the occurrence and development of gastric cancer(GC) has not been fully elucidated.AIM To explore the expression level and molecular mechanism of HOXD-AS2 in GC tissues and cells, and analyze its significance in the prognosis of GC.METHODS Real-time quantitative PCR was used to detect the expression of HOXD-AS2 in 79 pairs of GC tissues and five cell lines. The pc HOXD-AS2 plasmid vector was constructed and transfected into SGC-7901 and SNU-1 GC cells. Matrigel Transwell and wound healing assays were used to confirm the effect of HOXDAS2 on invasion and migration of GC cells. Cell counting kit-8 assay and flow cytometry were used to verify the effect of HOXD-AS2 on the proliferation, cell cycle, and apoptosis of GC cells. The relevant regulatory mechanism between HOXD-AS2 and HOXD8 and PI3K/Akt signaling pathway was verified by Western blot analysis.RESULTS The low expression of lncRNA HOXD-AS2 was associated with lymph node metastasis and tumor-node-metastasis stage in GC. In vitro functional experiments demonstrated that overexpression of HOXD-AS2 inhibited GC cell progression. Mechanistic studies revealed that HOXD-AS2 regulated the expression of its nearby gene HOXD8 and inhibited the activity of the PI3K/Akt signaling pathway.CONCLUSION These results indicate that downregulation of HOXD-AS2 significantly promotes the progression of GC cells by regulating HOXD8 expression and activating the PI3K/Akt signaling pathway. HOXD-AS2 may be a novel diagnostic biomarker and effective therapeutic target for GC.

Basic Study Long non-coding RNA TP73-AS1 promotes pancreatic cancer growth and metastasis through miRNA-128-3p/GOLM1 axis

BACKGROUND Previous studies have suggested that long non-coding RNAs(lncRNA)TP73-AS1 is significantly upregulated in several cancers.However,the biological role and clinical significance of TP73-AS1 in pancreatic cancer(PC)remain unclear.AIM To investigate the role of TP73-AS1 in the growth and metastasis of PC.METHODS The expression of lncRNA TP73-AS1,miR-128-3p,and GOLM1 in PC tissues and cells was detected by quantitative real-time polymerase chain reaction.The bioinformatics prediction software ENCORI was used to predict the putative binding sites of miR-128-3p.The regulatory roles of TP73-AS1 and miR-128-3p in cell proliferation,migration,and invasion abilities were verified by Cell Counting Kit-8,wound-healing,and transwell assays,as well as flow cytometry and Western blot analysis.The interactions among TP73-AS1,miR-128-3p,and GOLM1 were explored by bioinformatics prediction,luciferase assay,and Western blot.RESULTS The expression of TP73-AS1 and miRNA-128-3p was dysregulated in PC tissues and cells.High TP73-AS1 expression was correlated with a poor prognosis.TP73-AS1 silencing inhibited PC cell proliferation,migration,and invasion in vitro as well as suppressed tumor growth in vivo.Mechanistically,TP73-AS1 was validated to promote PC progression through GOLM1 upregulation by competitively binding to miR-128-3p.CONCLUSION Our results demonstrated that TP73-AS1 promotes PC progression by regulating the miR-128-3p/GOLM1 axis,which might provide a potential treatment strategy for patients with PC.

Long non-coding RNA highly up-regulated in liver cancer promotes exosome secretion

BACKGROUND Highly upregulated in liver cancer (HULC) is a long non-coding RNA (lncRNA) which has recently been identified as a key regulator in hepatocellular carcinoma (HCC) progression. However, its role in the secretion of exosomes from HCC cells remains unknown. AIM To explore the mechanism by which HULC promotes the secretion of exosomes from HCC cells. METHODS Serum and liver tissue samples were collected from 30 patients with HCC who had not received chemotherapy, radiotherapy, or immunotherapy before surgery. HULC expression in serum exosomes and liver cancer tissues of patients was measured, and compared with the data obtained from healthy controls and tumor adjacent tissues. The effect of HULC upregulation in HCC cell lines and the relationship between HULC and other RNAs were studied using qPCR and dualluciferase reporter assays. Nanoparticle tracking analysis was performed to detect the quantity of exosomes.RESULTS HULC expression in serum exosomes of patients with HCC was higher than that in serum exosomes of healthy controls, and HULC levels were higher in liver cancer tissues than in tumor adjacent tissues. The expression of HULC in serum exosomes and liver cancer tissues correlated with the tumor-node-metastasis (TNM) classification, and HULC expression in tissues correlated with that in serum exosomes. Upregulation of HULC promoted HCC cell growth and invasion and repressed apoptosis. Notably, it also facilitated the secretion of exosomes from HCC cells. Moreover, qPCR assays showed that HULC repressed microRNA-372-3p (miR-372-3p) expression. We also identified Rab11a as a downstream target of miR-372-3p. Dual-luciferase reporter assays suggested that miR-372-3p could directly bind both HULC and Rab11a. CONCLUSION Our findings illustrate the importance of the HULC/miR-372-3p/Rab11a axis in HCC and provide new insights into the molecular mechanism regulating the secretion of exosomes from HCC cells.

Expressions of Long Non-Coding RNAs in Carcinogenesis of Cervix: A Review

Long non-coding RNAs (lncRNAs) are transcripts longer than 200 nucleotides mostly transcribed by RNA which do not encode proteins. Previously, lncRNAs were considered transcriptional byproducts called “junk DNA” with no biological functions. There are many studies conducted on lncRNAs showing they are actively involved in regulation of epigenetic, transcriptional, and post-transcriptional events. Expressions of lncRNAs are more different in many malignant tumors than in benign tumors and normal tissue. Aberration of lncRNAs is responsible to promote or suppress tumorigenesis and cancer progression. Under different circumstances, lncRNAs exhibit their roles in carcinogenesis such as MALAT1 is responsible for intervening mRNA instability, HOTAIR, MALAT1, ANRIL, PVT1 links with miRNA and histonemodifying complexes, MEG3 associates with miRNA, CCAT2, MEG3, GAS5, UCA1 allies with c-Myc or P53 causing suppression of tumor or oncogenesis. Abnormal expressions of lncRNAs are noticed in gynecological cancers, such as cervical cancer, ovarian cancer, and endometrial cancer. Identification of cervical cancer associated lncRNAs is necessary to understand the molecular biogenesis of cancers. In this review, we summarized the foundation and function of the lncRNAs in terms of tumor progression, invasion, prognosis, apoptosis, metastasis, and chemo-resistance. This review will provide references to determine the clinical applications of lncRNAs as ideal diagnostic biomarkers or therapeutic targets in cervical cancers.

结直肠癌组织LncRNA MEG3、miR-31表达及与病理特征的相关性

目的探讨结直肠癌组织长链非编码RNA母系印记基因3(LncRNA MEG3)、微小RNA-31(miR-31)表达及与病理特征的相关性。方法选取2019年1月—2021年10月我院收治的85例结直肠癌,比较癌组织与癌旁组织LncRNA MEG3与miR-31表达,应用Pearson相关性分析探讨LncRNA MEG3与miR-31的关系,采用荧光素酶报告基因检测分析LncRNA MEG3靶向调控miR-31情况,并比较不同病理特征患者LncRNA MEG3与miR-31表达,应用Spearman分析探讨LncRNA MEG3、miR-31与病理特征的相关性。结果癌组织LncRNA MEG3表达低于癌旁组织,miR-31表达高于癌旁组织(P<0.01)。LncRNA MEG3与miR-31表达呈负相关(r=-0.718,P<0.01)。荧光素酶报告基因检测结果显示,LncRNA MEG3 mimic可明显抑制WT-miR-31的荧光素酶活性(P<0.05);LncRNA MEG3组SW480细胞中miR-31表达显著降低,anti-LncRNA MEG3组SW480细胞中miR-31表达显著升高(P<0.05)。不同T分期、N分期、M分期、分化程度患者LncRNA MEG3与miR-31表达比较差异有统计学意义(P<0.01)。LncRNA MEG3表达与T分期、N分期呈负相关(r=-0.737、-0.725,P<0.01),与分化程度呈正相关(r=0.824,P<0.01);miR-31表达与T分期、N分期呈正相关(r=0.830、0.748,P<0.01),与分化程度呈负相关(r=-0.742,P<0.01)。结论结直肠癌组织中LncRNA MEG3呈低表达,miR-31呈高表达,且LncRNA MEG3可特异性结合miR-31,负向调控miR-31表达,影响结直肠癌患者病理特征。

急性缺血性脑卒中患者血清长链非编码RNA母系表达基因3和Zeste同源物增强子-2表达与神经功能损伤的相关性分析

目的探讨长链非编码RNA(lncRNA)母系表达基因3(MEG3)与Zeste同源物增强子-2(EZH2)在急性缺血性脑卒中(AIS)患者血清中的表达水平及其与神经功能损伤之间的关系。方法选取延安市人民医院2021年1月至2022年11月收治的92例AIS患者为脑卒中组,92例健康体检者为对照组,根据NIHSS评分将脑卒中组患者分为致残性损伤组19例,非致残性损伤组73例。采用实时荧光定量聚合酶链式反应、酶联免疫吸附法分别检测血清lncRNAMEG3、EZH2水平。采用Spearman相关分析法进行AIS患者血清lncRNAMEG3、EZH2表达水平与美国国立卫生研究院卒中量表(NIHSS)评分之间的相关性分析;采用多因素Logistic回归分析AIS患者合并神经功能致残性损伤的影响因素,并绘制受试者工作特征(ROC)曲线分析血清lncRNA MEG3、EZH2水平对AIS患者合并神经功能致残性损伤的诊断价值。结果脑卒中组患者血清lncRNA MEG3、EZH2表达水平均高于对照组(t=11.817、11.542,P<0.05)。Spearman相关分析显示,AIS患者血清lncRNA MEG3、EZH2水平与NIHSS评分均呈正相关(r=0.540、0.603,P<0.01)。致残性损伤组体质量指数、吸烟史占比、甘油三酯、总胆固醇、同型半胱氨酸、发病-到院时间(ODT)、lncRNAMEG3、EZH2水平均高于非致残性损伤组(t/χ2=2.103、5.050、9.121、5.585、2.276、5.448、4.638、4.682,P<0.05)。多因素Logistic回归分析显示,甘油三酯、总胆固醇、lncRNA MEG3、EZH2以及ODT均是AIS患者合并神经功能致残性损伤的影响因素(OR=4.853、4.277、2.674、3.052、3.901,P<0.05)。lncRNA MEG3、EZH2联合诊断AIS患者合并神经功能致残性损伤的曲线下面积(AUC)大于lncRNAMEG3以及EZH2单独诊断的AUC(Z=2.626、2.954,P<0.01),敏感度、特异度分别为94.74%、82.15%。结论AIS患者血清lncRNA MEG3、EZH2水平均上升,与AIS患者神经功能损伤程度均正相关,可用作AIS患者合并神经功能致残性损伤的诊断指标,且联合诊断效果更好。

LncRNA MEG3与miR-31在结肠腺瘤-癌序列转化中的交互作用及意义

目的探究长链非编码RNA母系印记基因3(LncRNA MEG3)与微小RNA-31(miR-31)在结肠腺瘤-癌序列转化中的交互作用与意义。方法选取2016年6月-2018年8月手术切除的62例结肠腺瘤、62例结肠腺瘤癌前病变、62例结肠癌组织,均行实时定量PCR检测LncRNA MEG3、miR-31的相对表达量;分析LncRNA MEG3与miR-31表达在不同序列转化阶段的相关性;分析LncRNA MEG3与miR-31表达在结肠腺瘤-癌序列转化中的交互作用;分析LncRNA MEG3、miR-31表达与结肠癌患者病理特征的相关性;分析LncRNA MEG3、miR-31表达对结肠癌患者生存率与死亡危险度的影响。结果LncRNA MEG3相对表达量在结肠腺瘤-癌序列转化中呈逐渐下降趋势,miR-31相对表达量在结肠腺瘤-癌序列转化中呈逐渐升高趋势(P<0.01)。Pearson相关性分析显示,LncRNA MEG3与miR-31在结肠腺瘤、结肠腺瘤癌前病变、结肠癌组织中均呈负相关(r=-0.741、-0.753、-0.774,P<0.05)。LncRNA MEG3低表达与miR-31高表达在结肠腺瘤-癌序列转化中呈正向交互作用(OR=30.375,γ=2.244),为次相乘模型。LncRNA MEG3相对表达量与结肠癌患者临床分期、淋巴结转移呈负相关,与结肠癌组织分化程度呈正相关,miR-31相对表达量与结肠癌组织临床分期、淋巴结转移呈正相关,与结肠癌组织分化程度呈负相关(P<0.01)。LncRNA MEG3低表达结肠癌患者3年生存率低于高表达患者,3年内死亡危险度是高表达患者的7.000倍(95%CI:1.027,47.704,P<0.05);miR-31高表达结肠癌患者3年生存率低于低表达患者,3年内死亡危险度是低表达患者的4.810倍(95%CI:1.846,12.536,P<0.05,P<0.01)。结论LncRNA MEG3低表达与miR-31高表达在结肠腺瘤-癌序列转化中具有正向交互作用,且二者均与结肠癌患者病理特征、生存状况密切相关,能为临床制定治疗方案、预测预后提供有效信息。

长链非编码RNA MEG3对鼻咽癌细胞增殖和侵袭的影响

目的探究长链非编码RNA母系表达基因3(MEG3)对鼻咽癌细胞增殖和侵袭的影响。方法体外培养鼻咽癌细胞系5-8F、CNE-2,转染MEG3分为空白对照组(转染试剂转染)、阴性转染组(MEG3阴性对照质粒转染)、MEG3转染组(MEG3 mimis质粒转染)。实时定量PCR(qRT-PCR)检测MEG3 mRNA表达;MTT法检测细胞增殖情况;平板细胞克隆实验检测菌落形成情况;流式细胞仪检测细胞凋亡以及周期分布情况;裸鼠模型肿瘤形成实验评估体内肿瘤生长情况;蛋白免疫印迹法(WB)检测细胞中Snail、N-钙黏着蛋白(N-cadherin)、波形蛋白(Vimentin)、E-钙黏着蛋白(E-cadherin)蛋白表达情况。结果与正常鼻咽上皮细胞系NP69相比,5-8F、CNE-2细胞中MEG3 mRNA表达均降低(P<0.05)。在5-8F、CNE-2细胞中,与空白对照组、阴性转染组相比,MEG3转染组细胞中MEG3mRNA表达升高(P<0.05)。在5-8F、CNE-2细胞中,随着细胞培养时间延长,MEG3转染组细胞抑制率逐渐升高;同一时间点,与空白对照组、阴性转染组相比,MEG3转染组细胞抑制率均升高(P<0.05)。与空白对照组、阴性转染组相比,MEG3转染组细胞菌落数量、细胞迁移、侵袭数量均降低(P<0.05)。与空白组、阴性转染组对比,MEG3转染组细胞凋亡率、G1期DNA含量均升高,差异有统计学意义(P<0.05)。与空白组、阴性转染组对比,在1、2周MEG3转染组肿瘤体积均变小(P<0.05)。与空白组、阴性转染组相比,MEG3转染组Snail、N-cadherin、Vimentin蛋白表达均降低,E-cadherin蛋白表达升高(P<0.05)。结论 MEG3在鼻咽癌中表达降低,MEG3表达升高后可抑制鼻咽癌细胞的增殖、侵袭、迁移,使细胞周期停留在G1期,促进细胞凋亡,其机制可能与抑制上皮细胞-间充质转化有关。

LncRNA CCAT1通过PI3K/AKT信号通路影响子宫内膜癌细胞的增殖和凋亡

目的:探讨长链非编码RNA(LncRNA)CCAT1对子宫内膜癌细胞增殖、凋亡和磷脂酰肌醇3-激酶(PI3K)/蛋白激酶B(AKT)信号通路影响,阐明CCAT1在子宫内膜癌生长中的作用及可能机制。方法:将HEC-1-A细胞分为空白对照组(BC)、阴性对照组(NC)和CCAT1-siRNA组,CCAT1-siRNA组细胞转染CCAT1-siRNA,NC组转染阴性对照siRNA,BC组不转染。RT-PCR测定细胞中CCAT1水平。CCK8测定HEC-1-A细胞增殖情况。流式细胞术测定HEC-1-A细胞凋亡。Western blot测定HEC-1-A细胞PCNA、活化的cleaved caspase 3、Bax、Bcl-2、PI3K、AKT、p-AKT蛋白水平。结果:HEC-1-A细胞中CCAT1水平(2.15±0.24)高于T-HESC细胞(1.00±0.13)(t=11.147,P<0.001)。与BC组和NC组相比,CCAT1-siRNA组HEC-1-A细胞中CCAT1水平降低(P<0.001),细胞增殖率降低(P<0.001),细胞凋亡率降低(F=112.080,P<0.001),PCNA和Bcl-2蛋白水平降低(P<0.001),cleaved caspase 3和Bax蛋白水平升高(P<0.001),PI3K和p-AKT蛋白水平降低(P<0.001)。BC组和NC组HEC-1-A细胞中各指标差异无统计学意义(P>0.05)。结论:沉默子宫内膜癌细胞中CCAT1可抑制细胞增殖、促进细胞凋亡,其机制可能与沉默CCAT1可抑制PI3K/AKT信号通路有关。

LncRNA FTH1P3通过调控PI3K/AKT信号通路促进胃癌细胞增殖和迁移能力

目的 研究长链非编码RNA铁蛋白重链1伪基因3(LncRNA FTH1P3)在胃癌组织中的表达及临床意义,并探讨LncRNA FTH1P3通过调控磷脂酰肌醇3-激酶(PI3K)/苏氨酸蛋白激酶(AKT)信号通路促进胃癌细胞增殖和迁移的作用机制。方法 收集胃癌和癌旁组织标本,采用qRT-PCR检测LncRNA FTH1P3在胃癌组织中的表达,分析LncRNA FTH1P3的表达与胃癌患者病理参数和预后的关系。常规培养胃癌细胞,分为si-NC组和si-LncRNA FTH1P3-1组、si-LncRNA FTH1P3-2组,采用LncRNA FTH1P3 siRNA转染胃癌细胞,qRT-PCR检测各组细胞中LncRNA FTH1P3的表达;CCK8实验检测各组细胞增殖能力;Transwell实验检测各组细胞迁移能力;体内成瘤实验检测各组细胞体内成瘤能力;Western blot检测各组细胞PI3K/AKT信号通路相关蛋白PI3K、AKT、磷酸化PI3K(pPI3K)、磷酸化AKT(pAKT)的表达。结果 LncRNA FTH1P3在胃癌组织中表达上调(P<0.05)。LncRNA FTH1P3高表达与患者肿瘤最大径、分化程度、淋巴结转移情况和TNM分期有关(P<0.05)。与si-NC组相比,si-LncRNA FTH1P3-1组和si-LncRNA FTH1P3-2组胃癌细胞中LncRNA FTH1P3表达显著减少(P<0.05),si-LncRNA FTH1P3-1组和si-LncRNA FTH1P3-2组胃癌细胞增殖、迁移、体内成瘤能力显著降低(P<0.05);细胞中pPI3K和pAKT的表达减少(P<0.05)。结论 LncRNA FTH1P3通过调控PI3K/AKT信号通路促进胃癌细胞增殖及迁移,有望成为治疗胃癌的潜在分子靶点。

长链非编码RNA AC023794.4-201在喉鳞状细胞癌中的表达及临床意义

喉癌是头颈部最常见的恶性肿瘤之一,其中85%～95%为鳞状细胞癌（laryngeal squamous cell carcinoma,LSCC）[1]。据报道早期LSCC患者的生存率远高于晚期患者[2]。研究发现,长链非编码RNA（long non-coding RNA,lncRNA）参与调控头颈部肿瘤细胞的增殖、分化、迁移和侵袭等,发挥抑癌基因或癌基因的功能[3～5]。

LncRNA MAGI2-AS3导致鼻咽癌细胞放疗抵抗的作用机制研究

目的 研究长链非编码RNA含有WW和PDZ结构域2的膜相关鸟苷酸激酶反义RNA 3(LncRNA MAGI2-AS3)在鼻咽癌组织中的表达及与患者放射治疗(放疗)敏感性的关系,并探讨LncRNA MAGI2-AS3对鼻咽癌细胞放疗抵抗的影响及作用机制。方法 采用反转录荧光定量聚合酶链反应(RT-qPCR)检测LncRNA MAGI2-AS3在鼻咽癌组织中的表达水平,分析LncRNA MAGI2-AS3与鼻咽癌患者放疗敏感性的关系。常规培养鼻咽癌细胞CNE2,转染LncRNA MAGI2-AS3小干扰RNA(siRNA),根据是否转染siRNA分为si-NC组和si-LncRNA MAGI2-AS3组。采用CCK8实验检测各组细胞的放疗敏感性;放射处理后,采用平板克隆实验、流式细胞实验、裸鼠实验分别检测各组细胞克隆形成能力、细胞周期、凋亡情况和细胞体内生长能力;采用Western blot试验检测各组细胞周期蛋白D1(cyclin D1)、细胞周期蛋白依赖性激酶4(CDK4)、凋亡蛋白活化的含半胱氨酸的天冬氨酸蛋白水解酶(caspase)3、caspase9表达。结果 RT-qPCR检测结果显示,LncRNA MAGI2-AS3在鼻咽癌组织中表达上调(P<0.05)。LncRNA MAGI2-AS3高表达与患者放疗抵抗有关(P<0.05)。与si-NC组相比,si-LncRNA MAGI2-AS3组鼻咽癌细胞中LncRNA MAGI2-AS3表达减少、对放疗敏感性增加(P<0.05)。放射处理后,si-LncRNA MAGI2-AS3组鼻咽癌细胞克隆形成能力降低(P<0.05),细胞周期阻滞在G/G期(P<0.05),细胞凋亡增加(P<0.05),细胞体内生长能力显著降低(P<0.05),cyclin D1、CDK4表达降低,caspase3、caspase9表达增加(P<0.05)。结论 LncRNA MAGI2-AS3通过调控细胞周期和凋亡促进鼻咽癌细胞放疗抵抗,是逆转鼻咽癌放疗抵抗的潜在分子靶点。

长链非编码RNA MCM3AP-AS1对NSCLC细胞增殖、侵袭及迁移的影响

目的探讨长链非编码RNA(lncRNA)微小染色体维持蛋白3相关蛋白反义链1(MCM3AP-AS1)对非小细胞肺癌(NSCLC)细胞增殖、侵袭、迁移的影响及作用机制。方法体外培养A549肺癌细胞株,并将其分为空白对照(Control)组、阴性对照(NC)组、过表达MCM3AP-AS1组和敲低sh-MCM3AP-AS1组。NC组利用空载质粒转染A549肺癌细胞;过表达MCM3AP-AS1组利用lncRNA MCM3AP-AS1过表达质粒转染A549肺癌细胞;sh-MCM3AP-AS1组使用干扰RNA(siRNA)敲低lncRNA MCM3AP-AS1并转染A549肺癌细胞。采用实时荧光定量PCR(qRT-PCR)法检测lncRNA MCM3AP-AS1的相对表达量;CCK8实验检测肺癌细胞的增殖情况;Transwell和划痕实验检测肺癌细胞的侵袭和迁移情况。结果与Control组相比,NC组lncRNA MCM3AP-AS1水平及肺癌细胞增殖、侵袭和迁移情况均无明显变化(P>0.05),过表达MCM3AP-AS1组lncRNA MCM3AP-AS1水平及肺癌细胞增殖、侵袭和迁移均明显增强(P<0.05),sh-MCM3AP-AS1组lncRNA MCM3AP-AS1水平及肺癌细胞增殖、侵袭和迁移均明显减弱(P<0.05)。结论过表达NSCLC细胞中的lncRNA MCM3AP-AS1水平可促进肺癌细胞的增殖、侵袭及迁移;敲低NSCLC细胞中的lncRNA MCM3AP-AS1水平可抑制肺癌细胞的增殖、侵袭及迁移。

肝细胞癌患者血清PTPN3、VEGF、IRX5、HOTAIR的表达水平及其与病理特征和预后的相关性

目的检测血清蛋白质酪氨酸磷酸酶3(PTPN3)、血管内皮生长因子(VEGF)、易洛魁族同源盒基因5(IRX5)、长链非编码RNA HOX转录反义RNA(HOTAIR)在肝细胞癌(HCC)中的表达水平,并分析其与患者的病理特征和预后的相关性,为临床工作提供血清学参考。方法选取2020年6月至2022年10月南阳市中心医院收治的117例HCC患者作为观察组,另选取同期117例良性肝内结节患者作为对照组,比较两组患者的血清PTPN3、VEGF、IRX5、HOTAIR水平,分析HCC患者血清PTPN3、VEGF、IRX5、HOTAIR水平与病理特征的关系。随访6个月,依据患者预后情况分为预后良好组72例和预后不良组45例,比较不同预后患者的血清PTPN3、VEGF、IRX5、HOTAIR水平,采用受试者工作特征(ROC)曲线分析血清PTPN3、VEGF、IRX5、HOTAIR单独及联合预测HCC预后的效能,采用相对危险度(RR)分析血清PTPN3、VEGF、IRX5、HOTAIR水平与HCC预后的关系。结果观察组患者的血清PTPN3、VEGF、IRX5、HOTAIR水平分别为(181.42±10.19)ng/mL、(154.66±11.82)μmol/L、(82.42±8.23)ng/mL、1.20±0.28,明显高于对照组的(86.64±13.28)ng/m L、(83.64±9.50)μmol/L、(34.80±6.63)ng/m L、1.07±0.25,差异均有统计学意义(P<0.05);不同TNM分期、分化程度、肿瘤直径、伴肝硬化、区域淋巴结转移、Ki-67指数、脉管内瘤栓、包膜侵犯HCC患者血清PTPN3、VEGF、IRX5、HOTAIR水平比较,差异均有统计学意义(P<0.05);肿瘤多发患者的血清VEGF水平为(154.10±10.26)μmol/L,明显高于肿瘤单发患者的(191.62±9.45)μmol/L,差异有统计学意义(P<0.05);治疗后2个月,预后良好患者的血清PTPN3、VEGF、IRX5、HOTAIR水平分别为(153.69±22.24)ng/m L、(113.27±25.64)μmol/L、(70.53±10.24)ng/m L、1.15±0.23,明显低于预后不良患者的(217.58±27.06)ng/m L、(215.33±38.19)μmol/L、(96.35±14.88)ng/m L、1.36±0.28,差异均有统计学意义(P<0.05);绘制血清PTPN3、VEGF、IRX5、HOTAIR单独及联合预测HCC预后的ROC,结果显示各血清联合预测的AUC最大,为0.924(95%CI:0.860~0.965);HCC预后不良的危险度分析结果显示,血清PTPN3、VEGF、IRX5、HOTAIR所致RR值分别为4.604(95%CI:2.602~8.145)、7.139(95%CI:3.660~13.924)、4.733(95%CI:2.749~8.149)、4.690(95%CI:2.575~8.544)(P<0.05)。结论血清PTPN3、VEGF、IRX5、HOTAIR在HCC中的表达异常升高,且与病理特征联系密切,对患者预后有一定评估作用。

长链非编码RNA AC005154.6抑制前列腺癌PC-3细胞增殖和迁移的机制

目的检测长链非编码RNA AC005154.6在前列腺癌组织及细胞系的表达情况,探索上调AC005154.6抑制前列腺癌细胞增殖和迁移的分子机制。方法实时荧光定量PCR(RT-qPCR)检测AC005154.6在61例前列腺癌组织及癌旁组织和4种细胞系(PC-3、LNCap、C4-2B、DU-145)中的表达。将AC005154.6表达最低的细胞系按随机数字法分为对照组(感染携带无意义序列的重组慢病毒)和实验组(感染携带AC005154.6序列的重组慢病毒)。RT-qPCR检测感染效率。CCK-8法和划痕实验分别检测上调AC005154.6对细胞增殖能力和迁移能力的作用。RT-qPCR和Western blot分别检测上调AC005154.6对肿瘤坏死因子α诱导蛋白3(TNFAIP3)表达的作用。结果与癌旁组织比较,AC005154.6在前列腺癌组织表达下调(P<0.01)。与正常前列腺上皮细胞比较,AC005154.6在以上4种前列腺癌细胞系表达均下调(P<0.05),AC005154.6在PC-3细胞中的表达最低(P<0.01)。与对照组比较,实验组PC-3细胞中AC005154.6表达显著增加(P<0.01)。与对照组比较,实验组PC-3细胞的增殖能力显著下降(P<0.05),细胞迁移能力显著降低(P<0.01)。与对照组比较,实验组PC-3细胞中TNFAIP3表达显著增加(P<0.01)。结论AC005154.6在前列腺癌组织和细胞系中低表达,上调AC005154.6可抑制前列腺癌PC-3细胞的增殖和迁移能力,其分子机制可能与AC005154.6促进TNFAIP3基因的表达有关。

Upregulation of MEG3 inhibits neuroblastoma progression via decreasing proliferation and promoting apoptosis

Background:We have shown that downregulation of materally expressed gene 3(MEG3)promoted autophagy and epithelial-mesenchymal transition to promote neuroblastoma(NB)progression.In present study,we aim to further discover the role of MEG3 in NB.Methods:Expression levels of MEG3 in stabled transfected cells were detected by qPCR.Flow cytometry was used to examine the effects of MEG3 overexpression on apoptosis and cell cycle.Moreover,tumor stemness was detected by tumor sphere formation assay.Results:QPCR showed that MEG3 was successfully overexpressed in SK-N-BE(2)C and SK-N-AS cells.CCK8 indicated MEG3 reduced cell proliferation in two NB cells.Flow cytometry revealed that MEG3 promoted apoptosis and caused G0/G1 arrest.Using chromatin isolation by RNA purification(ChIRP)and tumor sphere formation assays,we revealed that upregulation of MEG3 decreased tumor stemness by decreasing Nestin transcription.Conclusions:Overall,present study confirmed an anti-cancer role of MEG3 in NB,demonstrated that MEG3 could be a potential therapeutic target of NB.

Danhongqing formula alleviates cholestatic liver fibrosis by downregulating long non-coding RNA H19 derived from cholangiocytes and inhibiting hepatic stellate cell activation

Objective:This study explores the mechanism of action of Danhongqing formula(DHQ),a compoundbased Chinese medicine formula,in the treatment of cholestatic liver fibrosis.Methods:In vivo experiments were conducted using 8-week-old multidrug resistance protein 2 knockout(Mdr2-/-)mice as an animal model of cholestatic liver fibrosis.DHQ was administered orally for 8 weeks,and its impact on cholestatic liver fibrosis was evaluated by assessing liver function,liver histopathology,and the expression of liver fibrosis-related proteins.Real-time polymerase chain reaction,Western blot,immunohistochemistry and other methods were used to observe the effects of DHQ on long non-coding RNA H19(H19)and signal transducer and activator of transcription 3(STAT3)phosphorylation in the liver tissue of Mdr2-/-mice.In addition,cholangiocytes and hepatic stellate cells(HSCs)were cultured in vitro to measure the effects of bile acids on cholangiocyte injury and H19 expression.Cholangiocytes overexpressing H19 were constructed,and a conditioned medium containing H19 was collected to measure its effects on STAT3 protein expression and cell activation.The intervention effect of DHQ on these processes was also investigated.HSCs overexpressing H19 were constructed to measure the impact of H19 on cell activation and assess the intervention effect of DHQ.Results:DHQ alleviated liver injury,ductular reaction,and fibrosis in Mdr2-/-mice,and inhibited H19expression,STAT3 expression and STAT3 phosphorylation.This formula also reduced hydrophobic bile acid-induced cholangiocyte injury and the upregulation of H19,inhibited the activation of HSCs induced by cholangiocyte-derived conditioned medium,and decreased the expression of activation markers in HSCs.The overexpression of H19 in a human HSC line confirmed that H19 promoted STAT3 phosphorylation and HSC activation,and DHQ was able to successfully inhibit these effects.Conclusion:DHQ effectively alleviated spontaneous cholestatic liver fibrosis in Mdr2-/-mice by inhibiting H19 upregulation in cholangiocytes and preventing the inhibition of STAT3 phosphorylation in HSC,thereby suppressing cell activation.

长链非编码RNA H19在小鼠溃疡性结肠炎相关结直肠癌发病过程中的作用研究

目的探讨小鼠溃疡性结肠炎相关结直肠癌(CAC)发病过程中,长链非编码RNA H19(H19)的表达和意义。方法将30只C57BL/6小鼠随机分成对照组和观察组。观察组小鼠用氧化偶氮甲烷/葡聚糖硫酸钠方式共同造模。对照组小鼠在相同时间给予腹腔内注射无菌生理盐水,同时饮用洁净水。第71天处死小鼠,比较两组小鼠结肠组织中H19、mRNA let-7a(let-7a)、p-Janus激酶2(p-JAK2)、p-转录激活因子3(p-STAT3)表达量的差异。结果观察组小鼠结肠组织中H19 mRNA表达量高于对照组(P<0.05),观察组小鼠结肠组织中let-7a mRNA表达量低于对照组(P<0.05)。观察组小鼠结肠组织中p-JAK2和p-STAT3蛋白表达水平高于对照组(P<0.05)。结论H19在小鼠结肠癌组织中的高表达伴随着STAT3表达增加,对CAC发病起到了推动的作用。

Expression Profile and Function Analysis of Long Non-coding RNAs in the Infection of Coxsackievirus B3

The roles of lnc RNAs in the infection of enteroviruses have been barely demonstrated. In this study, we used coxsackievirus B3(CVB3), a typical enterovirus, as a model to investigate the expression profiles and functional roles of lnc RNAs in enterovirus infection. We profiled lnc RNAs and m RNA expression in CVB3-infected He La cells by lnc RNA-m RNA integrated microarrays. As a result, 700 differentially expressed lnc RNAs(431 up-regulated and 269 down-regulated) and665 differentially expressed m RNAs(299 up-regulated and 366 down-regulated) were identified in CVB3 infection. Then we performed lnc RNA-m RNA integrated pathway analysis to identify potential functional impacts of the differentially expressed m RNAs, in which lnc RNA-m RNA correlation network was built. According to lnc RNA-m RNA correlation, we found that XLOC-001188, an lnc RNA down-regulated in CVB3 infection, was negatively correlated with NFAT5 m RNA,an anti-CVB3 gene reported previously. This interaction was supported by q PCR detection following si RNA-mediated knockdown of XLOC-001188, which showed an increase of NFAT5 m RNA and a reduction of CVB3 genomic RNA. In addition, we observed that four most significantly altered lnc RNAs, SNHG11, RP11-145 F16.2, RP11-1023 L17.1 and RP11-1021 N1.2 share several common correlated genes critical for CVB3 infection, such as BRE and IRF2 BP1. In all, our studies reveal the alteration of lnc RNA expression in CVB3 infection and its potential influence on CVB3 replication,providing useful information for future studies of enterovirus infection.