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Coordinated silencing of the Sp1-mediated long noncoding RNA MEG3 by EZH2 and HDAC3 as a prognostic factor in pancreatic ductal adenocarcinoma

机译:通过EzH2和HDAC3协调SP1介导的长非致rna Meg3的沉默作为胰腺导管腺癌的预后因子

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摘要

Objective:Pancreatic ductal adenocarcinoma(PDAC)is a disease with high mortality.Many so-called"junk"noncoding RNAs need to be discovered in PDAC.The purpose of this study was therefore to investigate the function and regulatory mechanism of the long noncoding RNA MEG3 in PDAC.Methods:The Gene Expression Omnibus database(GEO database)was used to determine the differential expression of long noncoding RNAs in PDAC,and MEG3 was selected for subsequent verification.Tissue and cell samples were used to verify MEG3 expression,followed by functional detection in vitro and in vivo.Microarrays were used to characterize long noncoding RNA and mRNA expression profiles.Competing endogenous RNA analyses were used to detect differential MEG3 and relational miRNA expression in PDAC.Finally,promoter analyses were conducted to explain the downregulation of MEG3 PDAC.Results:We generated a catalogue of PDAC-associated long noncoding RNAs in the GEO database.The ectopic expression of MEG3 inhibited PDAC growth and metastasis in vitro and in vivo,which was statistically significant(P<0.05).Microarray analysis showed that multiple microRNAs interacted with MEG3.We also showed that MEG3,as a competing endogenous RNA,directly sponged miR-374a-5p to regulate PTEN expression.The transcription factor,Sp1,recruited EZH2 and HDAC3 to the promoter and transcriptionally repressed MEG3 expression.Finally,clinical data showed that MEG3 and miR-374a-5p expressions were correlated with clinicopathological features.Statistically,Sp1,EZH2,HDAC3,and miR-374 a-5p were negatively correlated with MEG3(P<0.05).Conclusions:Reduced MEG3 levels played a crucial role in the PDAC malignant phenotype,which provided insight into novel and effective molecular targets of MEG3 for pancreatic cancer treatment.
机译:目的:胰腺导管腺癌(PDAC)是一种患有高死亡率的疾病。因此,在PDAC中需要发现所谓的“垃圾”非编码RNA。因此,本研究的目的是探讨长非数性RNA的功能和调节机制Meg3在pdac.m.methods:基因表达omnibus数据库(Geo数据库)用于确定PDAC中长的非分量RNA的差异表达,并选择MEG3用于后续验证。使用和细胞样品用于验证MEG3表达,然后用于验证MEG3表达,然后用于验证MEG3表达,然后使用在体外和体内的功能性检测用于表征长的非分量RNA和mRNA表达谱所以使用内源性RNA分析来检测PDAC的差异MEG3和关系miRNA表达。进行启动子分析以解释MEG3的下调。解释MEG3的下调pdac.results:我们在Geo数据库中生成了PDAC相关的长非编码RNA的目录。MEG3的异位表达抑制了PDAC体外和体内生长和转移,其统计学显着(P <0.05).microarray分析表明,多个microRNAs与meg3相互作用。我们还表明Meg3,作为竞争内源性RNA,直接冲压miR-374a-5p来调节PTEN表达。转录因子,SP1,募集EZH2和HDAC3至启动子和转录抑制的MEG3表达。最后,临床资料显示MEG3和MIR-374A-5P表达与临床病理特征相关。,SP1,EZH2,HDAC3, MiR-374 A-5P与MEG3负相关(P <0.05)。结论:降低的MEG3水平在PDAC恶性表型中发挥了至关重要的作用,该表型在PDAC恶性表型中发挥了重要作用,这提供了对胰腺癌治疗的新颖和有效分子靶标的洞察力。

著录项

  • 来源
    《癌症生物学与医学:英文版》 |2020年第004期|P.953-969|共17页
  • 作者单位

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

    Department of Pathology Fudan University Eye Ear Nose and Throat Hospital Shanghai 201114 China;

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

    Shanghai Center for Bioinformation Technology Shanghai 201203 China;

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 ChinaState Key Laboratory of Oncogenes and Related Genes Shanghai Cancer Institute Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

    Department of Oncology Renji Hospital School of Medicine Shanghai Jiaotong University Shanghai 200127 China;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 chi
  • 中图分类 肿瘤学;
  • 关键词

    Pancreatic ductal adenocarcinoma; MEG3; Sp1; EZH2; HDAC3; miR-374a-5p;

    机译:胰腺导管腺癌;MEG3;SP1;EZH2;HDAC3;MIR-374A-5P;
  • 入库时间 2022-08-19 04:55:52
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