Long non-coding RNA GATA6-AS1 is mediated by N6-methyladenosine methylation and inhibits the proliferation and metastasis of gastric cancer

BACKGROUND Through experimental research on the biological function of GATA6-AS1,it was confirmed that GATA6-AS1 can inhibit the proliferation,invasion,and migration of gastric cancer cells,suggesting that GATA6-AS1 plays a role as an anti-oncogene in the occurrence and development of gastric cancer.Further experi-ments confirmed that the overexpression of fat mass and obesity-associated protein(FTO)inhibited the expression of GATA6-AS1,thereby promoting the occurrence and development of gastric cancer.AIM To investigate the effects of GATA6-AS1 on the proliferation,invasion and migration of gastric cancer cells and its mechanism of action.METHODS We used bioinformatics methods to analyze the Cancer Genome Atlas(https://portal.gdc.cancer.gov/.The Cancer Genome Atlas)and download expression data for GATA6-AS1 in gastric cancer tissue and normal tissue.We also constructed a GATA6-AS1 lentivirus overexpression vector which was transfected into gastric cancer cells to investigate its effects on proliferation,migration and invasion,and thereby clarify the expression of GATA6-AS1 in gastric cancer and its biological role in the genesis and development of gastric cancer.Next,we used a database(http://starbase.sysu.edu.cn/starbase2/)to analysis GATA6-AS1 whether by m6A methylation modify regulation and predict the methyltransferases that may methylate GATA6-AS1.Furthermore,RNA immunoprecipitation experiments confirmed that GATA6-AS1 was able to bind to the m6A methylation modification enzyme.These data allowed us to clarify the ability of m6A methylase to influence the action of GATA6-AS1 and its role in the occurrence and development of gastric cancer.RESULTS Low expression levels of GATA6-AS1 were detected in gastric cancer.We also determined the effects of GATA6-AS1 overexpression on the biological function of gastric cancer cells.GATA6-AS1 had strong binding ability with the m6A demethylase FTO,which was expressed at high levels in gastric cancer and negatively correlated with the expression of GATA6-AS1.Following transfection with siRNA to knock down the expression of FTO,the expression levels of GATA6-AS1 were up-regulated.Finally,the proliferation,migration and invasion of gastric cancer cells were all inhibited following the knockdown of FTO expression.CONCLUSION During the occurrence and development of gastric cancer,the overexpression of FTO may inhibit the expression of GATA6-AS1,thus promoting the proliferation and metastasis of gastric cancer.

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 noncoding RNAs HAND2-AS1 ultrasound microbubbles suppress hepatocellular carcinoma progression by regulating the miR-873-5p/tissue inhibitor of matrix metalloproteinase-2 axis

BACKGROUND Increasing data indicated that long noncoding RNAs(lncRNAs)were directly or indirectly involved in the occurrence and development of tumors,including hepatocellular carcinoma(HCC).Recent studies had found that the expression of lncRNA HAND2-AS1 was downregulated in HCC tissues,but its role in HCC progression is unclear.Ultrasound targeted microbubble destruction mediated gene transfection is a new method to overexpress genes.AIM To study the role of ultrasound microbubbles(UTMBs)mediated HAND2-AS1 in the progression of HCC,in order to provide a new reference for the treatment of HCC.METHODS In vitro,we transfected HAND2-AS1 siRNA into HepG2 cells by UTMBs,and detected cell proliferation,apoptosis,invasion and epithelial-mesenchymal transition(EMT)by cell counting kit-8 assay,flow cytometry,Transwell invasion assay and Western blotting,respectively.In addition,we transfected miR-837-5p mimic into UTMBs treated cells and observed the changes of cell behavior.Next,the UTMBs treated HepG2 cells were transfected together with miR-837-5p mimic and tissue inhibitor of matrix metalloproteinase-2(TIMP2)overexpression vector,and we detected cell proliferation,apoptosis,invasion and EMT.In vivo,we established a mouse model of subcutaneous transplantation of HepG2 cells and observed the effect of HAND2-AS1 silencing on tumor formation ability.RESULTS We found that UTMBs carrying HAND2-AS1 restricted cell proliferation,invasion,and EMT,encouraged apoptosis,and HAND2-AS1 silencing eliminated the effect of UTMBs.Additionally,miR-873-5p targets the gene HAND2-AS1,which also targets the 3’UTR of TIMP2.And miR-873-5p mimic counteracted the impact of HAND2-AS1.Further,miR-873-5p mimic solely or in combination with pcDNA-TIMP2 had been transformed into HepG2 cells exposed to UTMBs.We discovered that TIMP2 reversed the effect of miR-873-5p mimic caused by the blocked signalling cascade for matrix metalloproteinase(MMP)2/MMP9.In vivo results showed that HAND2-AS1 silencing significantly inhibited tumor formation in mice.CONCLUSION LncRNA HAND2-AS1 promotes TIMP2 expression by targeting miR-873-5p to inhibit HepG2 cell growth and delay HCC progression.

LncRNA LBX2-AS1在结肠癌中生物信息学分析及初步验证

目的基于生物信息学角度探讨长链非编码RNA(LncRNA)LBX2反义RNA1(LBX2-AS1)对结肠癌预后的影响并进行初步验证。方法在基因表达交互分析(GEPIA)数据库查找并明确与结肠癌预后密切相关的基因LBX2-AS1,在UCSCxena数据库中下载结肠癌数据集(TCGA-COAD)及生存信息,并分为LBX2-AS1高低表达组后绘制生存曲线。分别检测临床标本结肠癌及癌旁组织中LBX2-AS1的表达并分析其与结肠癌临床病理特征的相关性。沉默SW480细胞株LBX2-AS1表达后,通过细胞增殖实验、细胞划痕实验、Transwell侵袭实验检测各组细胞的增殖、侵袭和转移能力。结果通过GEPIA数据库检索发现LBX2-AS1与结肠癌患者的预后密切相关。UCSCxena数据库下载TCGA-COAD的生存信息分析提示,随着生存时间延长,高表达LBX2-AS1组存活例数明显少于低表达组;与癌旁组织比较,LBX2-AS1在结肠癌组织中明显高表达,且表达水平与患者年龄、性别临床参数无关,与结肠癌的病理分期及淋巴结转移呈正相关。沉默LBX2-AS1后结肠癌细胞SW480细胞增殖率明显降低,划痕距离明显增宽,侵袭细胞数明显减少,差异有统计学意义(P<0.05)。结论基于生物信息学分析,结合临床数据及细胞实验验证,LncRNA LBX2-AS1在结肠癌中起促癌作用。

布比卡因调控LncRNA LBX2-AS1对宫颈癌细胞SiHa增殖及凋亡的影响

目的:探讨布比卡因对宫颈癌细胞SiHa增殖、凋亡的影响及其对LncRNA LBX2-AS1的调控作用。方法:体外培养人宫颈癌细胞SiHa,分别加入不同剂量的布比卡因处理细胞,分别将si-NC、si-LBX2-AS1转染至SiHa细胞,分别将pcDNA、pcDNA-LBX2-AS1转染至SiHa细胞后使用布比卡因处理;采用MTT实验检测细胞增殖;应用流式细胞仪检测细胞周期及细胞凋亡率;采用qRT-PCR法检测LBX2-AS1的表达量;Western blot法检测Cleaved-caspase3、pro-caspase3蛋白表达量。结果:布比卡因可明显降低光密度(OD)值、S期细胞比例、LBX2-AS1的表达水平及pro-caspase3蛋白水平(P<0.05),提高凋亡率、G0-G1期细胞比例及Cleaved-caspase3蛋白水平(P<0.05);转染si-LBX2-AS1可明显降低OD值、S期细胞比例及pro-caspase3蛋白水平(P<0.05),提高凋亡率、G0-G1期细胞比例及Cleaved-caspase3蛋白水平(P<0.05);转染pcDNA-LBX2-AS1可明显逆转布比卡因对SiHa细胞增殖、细胞周期及凋亡的作用(P<0.05)。结论:布比卡因可通过下调LBX2-AS1的表达从而抑制宫颈癌细胞增殖、诱导细胞周期阻滞于G0-G1期细胞比例及促进细胞凋亡。

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.

长链非编码RNA LBX2-AS1调控微小RNA-491-5p影响骨肉瘤细胞增殖及凋亡的机制

目的探讨长链非编码RNA((lncRNA)LBX2-AS1靶向调控微小RNA(miRNA,miR)-491-5p影响骨肉瘤细胞增殖及凋亡的分子机制。方法采用实时定量反转录聚合酶链反应(RT-qPCR)检测2017年10月至2018年12月郑州大学第一附属医院收集的骨肉瘤组织与瘤旁组织中LBX2-AS1、miR-491-5p的表达量。选取人骨肉瘤细胞U2OS为研究对象,按照数字表法随机分为4组:si-NC组(转染si-NC)、si-LBX2-AS1组(转染si-LBX2-AS1)、si-LBX2-AS1+anti-miR-NC组(共转染si-LBX2-AS1与anti-miR-NC)、si-LBX2-AS1+anti-miR-491-5p组(共转染si-LBX2-AS1与anti-miR-491-5p),分别将si-NC、si-LBX2-AS1、si-LBX2-AS1与anti-miR-NC、si-LBX2-AS1与anti-miR-491-5p转染至U2OS细胞。噻唑蓝(MTT)检测细胞存活率;应用流式细胞仪检测细胞周期;流式细胞术检测细胞凋亡率;双荧光素酶报告实验验证LBX2-AS1与miR-491-5p的靶向关系;蛋白质印迹法(Western blot)检测细胞周期蛋白1(Cyclin D1)、p21、含半胱氨酸的天冬氨酸蛋白水解酶3(Caspase-3)蛋白表达量。两组间比较采用t检验,多组间比较采用单因素方差分析。结果瘤旁组织与骨肉瘤组织组织中LBX2-AS1的表达量分别为(1.01±0.10)、(3.56±0.35),miR-491-5p的表达量分别为(1.02±0.10)、(0.16±0.02),与瘤旁组织比较,骨肉瘤组织中LBX2-AS1的表达水平显著升高(t=35.027,P<0.05),miR-491-5p的表达水平显著降低(t=42.165,P<0.05),差异均有统计学意义;si-NC组与si-LBX2-AS1组细胞存活率分别为(100.02±10.00)%、(55.67±5.54)%,G1期比例分别为(38.51±2.55)%、(52.27±4.68)%,S期比例分别为(30.10±2.14)%、(15.36±1.26)%,细胞凋亡率分别为(8.28±0.92)%、(24.11±2.37)%,与si-NC组比较,si-LBX2-AS1组细胞存活率显著降低(t=11.638,P<0.05),细胞周期G1期比例明显升高(t=7.745,P<0.05),S期比例明显降低(t=17.806,P<0.05),细胞凋亡率显著升高(t=18.680,P<0.05),Cyclin D1表达量显著降低(t=20.871,P<0.05),p21、Caspase-3表达量显著升高(t=22.687,P<0.05;t=20.871,P<0.05),差异均有统计学意义;双荧光素酶报告实验证实LBX2-AS1能够靶向结合miR-491-5p;抑制miR-491-5p表达能减弱抑制LBX2-AS1表达对U2OS细胞增殖的抑制作用,还能减弱抑制LBX2-AS1表达对U2OS细胞凋亡的促进作用。结论lncRNA LBX2-AS1通过调控miR-491-5p从而促进骨肉瘤细胞增殖,抑制细胞凋亡。

LncRNA AFAP1-AS1 exhibits oncogenic characteristics and promotes gemcitabine-resistance of cervical cancer cells through miR-7-5p/EGFR axis

Background:Drug resistance is the main factor contributing to cancer recurrence and poor prognosis.Exploration of drug resistance-related mechanisms and effective therapeutic targets are the aim of molecular targeted therapy.In our study,the role of long non-coding RNA(lncRNA)AFAP1-AS1 in gemcitabine resistance and related mechanisms were explored in cervical cancer cells.Methods:Gemcitabine-resistant cervical cancer cell lines HT-3-Gem and SW756-Gem were constructed using the gemcitabine concentration gradient method.The overall survival rates and recurrence-free survival rates were evaluated by Kaplan-Meier analysis.The interaction was verified through a Dual-luciferase reporter gene assay and a Biotinylated RNA pull-down assay.Cell proliferation ability was assessed through methyl-thiazolyl-tetrazolium(MTT),soft agar,and colony formation experiments.Cell cycle and apoptosis were detected byflow cytometry.Results:Up-regulation of AFAP1-AS1 in cervical cancer predicted a poor prognosis.Besides,patients in the gemcitabine-resistance group had higher levels of AFAP1-AS1 than the gemcitabine-sensitive group.AFAP1-AS1 promoted tumor growth and induced gemcitabine tolerance of cervical cancer cells.In addition,AFAP1-AS1 mediated epidermal growth factor receptor(EGFR)expression by serving as a molecular sponge for microRNA-7a-5p(miR-7-5p).This present study also proved that the knockdown of EGFR or overexpression of miR-7a-5p abolished the accelerative role of AFAP1-AS1 overexpression in cancer progression and gemcitabine tolerance.Conclusions:In general,the AFAP1-AS1/miR-7-5p/EGFR axis was tightly related to the progression and gemcitabine tolerance of cervical cancer,providing potential targets for the management of cervical cancer.

长链非编码RNA LBX2-AS1通过表皮生长因子受体信号通路调控胶质瘤细胞增殖、迁移及凋亡的研究

目的探讨长链非编码RNA(lncRNA)LBX2-AS1通过表皮生长因子受体(EGFR)信号通路调控胶质瘤细胞增殖、迁移及凋亡的机制。方法2018年4月至2021年8月,将脑胶质瘤U251细胞(简称U251细胞)分为对照组和观察组,每组4株,对照组采用常规培养,观察组利用靶向LBX2-AS1的特异性小干扰RNA(siRNA)转染。采用四甲基偶氮唑盐法检测U251细胞增殖能力,划痕实验检测U251细胞转移率,流式细胞仪检测U251细胞凋亡率,蛋白印迹法检测U251细胞总蛋白及血管内皮生长因子(VEGF)、磷酸化磷酸肌醇3激酶(p-PI3K)、磷酸化蛋白激酶B(p-Akt)、磷酸化Ras(p-Ras)和磷酸化Raf(p-Raf)蛋白的表达。结果观察组U251细胞增殖能力、转移率明显低于对照组[(27.15±1.38)%比(63.54±2.47)%、(37.09±3.74)%比(82.17±9.24)%],U251细胞凋亡率明显高于对照组[(69.17±5.83)%比(17.58±1.22)%],差异有统计学意义(P<0.01)。观察组U251细胞总蛋白及VEGF、p-PI3K、p-Akt、p-Ras、p-Raf蛋白表达水平明显低于对照组(1.52±0.23比2.39±0.31、0.73±0.08比1.68±0.45、0.57±0.11比1.89±0.31、0.68±0.06比1.74±0.51、0.84±0.12比1.99±0.63和0.71±0.08比1.52±0.37),差异有统计学意义(P<0.01)。结论lncRNA LBX2-AS1在胶质瘤细胞中高表达,沉默lncRNA LBX2-AS1的表达通过EGFR通路抑制脑胶质瘤细胞的增殖和转移。