环状RNA hsa_circ_0012779在鼻咽癌中的表达及其对细胞生物学行为影响的机制研究

背景与目的:环状RNA(circular RNA,circRNA)在多种肿瘤的发展过程中发挥重要的调节作用。然而,circRNA在鼻咽癌中的异常表达和生物学功能仍不清楚。本研究旨在探讨hsa_circ_0012779对鼻咽癌细胞生物学行为的影响及其分子机制。方法:通过实时荧光定量聚合酶链反应(real-time fluorescence quantitative polymerase chain reaction,RTFQPCR)检测正常人鼻咽上皮细胞NP69及鼻咽癌细胞系CNE2、5-8F、HNE1、SUNE1中hsa_circ_0012779的表达。采用细胞计数试剂盒-8(cell counting kit-8,CCK-8)实验和transwell侵袭实验检测hsa_circ_0012779对鼻咽癌细胞增殖和侵袭能力的影响。采用蛋白质印迹法(Western blot)检测hsa_circ_0012779对ELAV样蛋白1(ELAV like protein 1,ELAVL1)表达的影响,通过RNA下拉实验验证hsa_circ_0012779与ELAVL1的直接结合。结果:hsa_circ_0012779在鼻咽癌组织和细胞中高表达,敲减hsa_circ_0012779能抑制鼻咽癌细胞增殖和侵袭,hsa_circ_0012779与RNA结合蛋白ELAVL1结合促进其表达并且共定位于细胞质中。同时,敲减hsa_circ_0012779对鼻咽癌细胞的影响能被ELAVL1过表达逆转。结论:hsa_circ_0012779促进ELAVL1的表达,进而促进鼻咽癌细胞增殖和侵袭,影响鼻咽癌的发生、发展。

circRNA001653对急性心肌梗死心肌细胞凋亡的作用及机制

目的探讨环状RNA(circRNA)_001653(circ_001653)对急性心肌梗死(AMI)心肌细胞凋亡的作用及机制。方法采用生物信息学分析AMI时差异表达的circRNA;大鼠心肌细胞分别培养于常氧(Normoxia组)和缺氧12 h(Hypoxia 12 h组)、24 h(Hypoxia 24 h组)、48 h(Hypoxia 48 h组)条件下,实时荧光定量PCR(RT-qPCR)检测上述4组细胞中circ_001653、微小RNA(microRNA)-324-5p、ELAV样RNA结合蛋白1(ELAVL1)的表达;选取缺氧48 h的心肌细胞转染sh-NC(sh-NC组)、sh-circ_001653(sh-circ_001653组)、circ-NC(circ-NC组)、circ_001653(circ_001653组)、miR-NC(miR-NC组)、miR-324-5p mimic(miR-324-5p mimic组)、circ_001653+miR-NC(circ_001653+miR-NC组)、circ_001653+miR-324-5p mimic(circ_001653+miR-324-5p mimic组)、miR-324-5p mimic+pcDNA3.1(miR-324-5p mimic+pcDNA3.1组)及miR-324-5p mimic+ELAVL1(miR-324-5p mimic+ELAVL1组)等载体,采用比色试剂盒和流式细胞术分别检测Normoxia组、Hypoxia-48 h组、sh-NC组、sh-circ_001653组、circ-NC组、circ_001653组、miR-NC组、miR-324-5p mimic组、circ_001653+miR-NC组、circ_001653+miR-324-5p mimic组、miR-324-5p mimic+pcDNA3.1组、miR-324-5p mimic+ELAVL1组心肌细胞中天冬氨酸特异性半胱氨酸蛋白酶-3(Caspase-3)、Caspase-9活性及细胞凋亡水平。结果生物信息学分析结果显示,与正常组比较、circ_001653在AMI中表达增强(P<0.05);与Normoxia组比较,Hypoxia 48 h组细胞中circ_001653和ELAVL1表达升高、miR-324-5p表达降低(P<0.05);与Normoxia组比较,Hypoxia 48 h组细胞凋亡率与Caspase-3、Caspase-9活力均升高(P<0.05);与sh-NC组比较,sh-circ_001653组细胞凋亡率和Caspase-3、Caspase-9活力均降低(P<0.05);与circ-NC组比较,circ_001653组细胞凋亡率和Caspase-3、Caspase-9活力均升高(P<0.05);与circ_001653+miR-NC组比较,circ_001653+miR-324-5p mimic组细胞凋亡率和Caspase-3、Caspase-9活力均降低(P<0.05);与miR-NC组比较,miR-324-5p mimic组细胞凋亡率和Caspase-3、Caspase-9活力均降低(P<0.05);与miR-324-5p mimic+pcDNA3.1组比较,miR-324-5p mimic+ELAVL1组细胞凋亡率和Caspase-3、Caspase-9活力升高(P<0.05)。结论circ_001653可促进AMI心肌细胞凋亡,其机制可能与circ_001653/miR-324-5p/ELAVL1轴作用有关。

卵巢浆液性肿瘤组织中类胚胎致死性异常视觉基因1、HCCR、MCM4的表达分析

探讨卵巢浆液性肿瘤组织中类胚胎致死性异常视觉基因1(ELAV1)、HCCR、MCM4的表达。方法:我院选择接受治疗的卵巢浆液性肿瘤患者60例开展研究,依据病理特点分成良性组与恶性组。观察两组患者的ELAV1、HCCR、MCM4表达情况。结果:卵巢浆液性恶性肿瘤组患者ELAV1、HCCR、MCM4阳性表达率明显较高,临床分期是为Ⅲ+Ⅳ期、组织学分级是中、低分化、有淋巴结转移的患者其蛋白阳性表达水平过高,年龄不同的患者其蛋白表达差异不显著,自变量以单因素为主,对蛋白水平行多因素分析,结果是组织学分级是影响卵巢浆液性恶性肿瘤蛋白水平的主要影响原因。结论:卵巢浆液性肿瘤患者的ELAV1、HCCR、MCM4阳性表达率较高,容易受患者组织学分级影响。

类胚胎致死性异常视觉基因1表达与卵巢浆液性癌化疗耐药及预后关系研究

目的探讨类胚胎致死性异常视觉基因1(ELAV1)在卵巢浆液性肿瘤组织中的表达与卵巢浆液性癌化疗耐药及预后的关系。方法采用免疫组化法对2010年1月至2013年2月中国医科大学附属盛京医院收治的40例卵巢浆液性癌(化疗耐药20例和化疗敏感20例)、15例卵巢交界性浆液性瘤、20例卵巢良性浆液性瘤及15例正常卵巢组织中的ELAV1蛋白表达进行检测,并对ELAV1表达与患者临床病理资料及生存率的关系进行分析。结果 (1)ELAV1蛋白胞浆在卵巢浆液性癌中的阳性表达率明显高于卵巢交界性浆液性瘤、卵巢良性浆液性瘤和正常卵巢组织(P<0.05),且在卵巢癌化疗耐药组织中明显高于化疗敏感组织(P<0.05)。(2)ELAV1蛋白胞核阳性表达率在卵巢浆液性癌、卵巢交界性浆液性瘤、卵巢良性浆液性瘤及正常卵巢组织中差异无统计学意义(P>0.05)。(3)胞浆ELAV1的表达与卵巢浆液性癌FIGO病理分期及淋巴结转移情况相关(P<0.05),与患者年龄、是否绝经及分化程度无关(P>0.05)。(4)Kaplan-Meier生存分析提示:ELAV1蛋白胞浆阳性和化疗耐药患者生存时间短。结论 ELAV1可能与卵巢浆液性癌的发生发展相关,可作为预测卵巢浆液性癌化疗耐药及预后的指标。

Long noncoding RNA 1392 regulates MDA5 by interaction with ELAVL1 to inhibit coxsackievirus B5 infection

Long noncoding RNAs(lncRNAs)modulate many aspects of biological and pathological processes.Recent studies have shown that host lncRNAs participate in the antiviral immune response,but functional lncRNAs in coxsackievirus B5(CVB5)infection remain unknown.Here,we identified a novel cytoplasmic lncRNA,LINC1392,which was highly inducible in CVB5 infected RD cells in a time-and dose-dependent manner,and also can be induced by the viral RNA and IFN-β.Further investigation showed that LINC1392 promoted several important interferon-stimulated genes(ISGs)expression,including IFIT1,IFIT2,and IFITM3 by activating MDA5,thereby inhibiting the replication of CVB5 in vitro.Mechanistically,LINC1392 bound to ELAV like RNA binding protein 1(ELAVL1)and blocked ELAVL1 interaction with MDA5.Functional study revealed that the 245–835 nt locus of LINC1392 exerted the antiviral effect and was also an important site for ELAVL1 binding.In mice,LINC1392 could inhibit CVB5 replication and alleviated the histopathological lesions of intestinal and brain tissues induced by viral infection.Our findings collectively reveal that the novel LINC1392 acts as a positive regulator in the IFN-I signaling pathway against CVB5 infection.Elucidating the underlying mechanisms on how lncRNA regulats the host innate immunity response towards CVB5 infection will lay the foundation for antiviral drug research.