一项独立预后因素分析snoRNA SCARNA4通过促进肺腺癌细胞增殖、迁移与侵袭驱动肿瘤进展并预示不良预后:基于功能验证与临床队列的研究OA
SnoRNA SCARNA4 as an independent prognostic factor drives tumor progression by promoting lung adenocarcinoma cell proliferation,migration and invasion and predicts poor prognosis:a functional validation and clinical cohort study
目的 分析小核仁RNA(small nucleolar RNA,snoRNA)在肺腺癌中的差异表达及其与患者预后的关联,筛选并验证肺腺癌相关snoRNA,探究其在肺腺癌发生发展中的作用机制.方法 采用Arraystar Small RNA表达芯片技术筛选肺腺癌组织与正常组织中差异表达的snoRNA,将芯片检测结果通过基因表达综合数据库(Gene Expression Omnibus,GEO)中GSE261702数据集验证后,筛选出通过分子克隆实验的snoRNA,并将上述snoRNA利用RT-qPCR进行验证;构建SCARNA4过表达模型(Vector组和SCARNA4组)和敲低模型(siNC组和si SCARNA4组),利用增殖、迁移及侵袭实验验证SCARNA4在肺腺癌细胞中的生物学功能;基于2013年2月至2015年5月陆军军医大学第二附属医院胸外科的108例肺腺癌患者的癌组织标本,通过RT-qPCR检测其SCARNA4表达水平,并运用X-tile软件确定最佳截断值,将患者分为SCARNA4高表达组与低表达组,绘制Kaplan-Meier曲线及构建Cox比例风险回归模型,分析SCARNA4表达水平对患者预后的影响.结果 Small RNA芯片检测结果获得在肺腺癌组织中表达上调的snoRNA共62条,表达下调的snoRNA有4条,通过GEO数据库及分子克隆实验成功获得8条候选snoRNA,RT-qPCR验证结果显示,与正常组织相比,SCARNA4在肺腺癌组织中的表达显著上调(P=0.042 7);过表达SCARNA4明显促进A549细胞的增殖、迁移及侵袭能力(P<0.001);敲低SCARNA4则显著抑制A549 细胞的增殖、迁移及侵袭能力(P<0.001).根据最佳截断值(3.48),将患者分为SCARNA4高表达组(57例)和SCARNA4低表达组(51例).Kaplan-Meier生存分析结果表明,高表达组患者的总生存期显著短于低表达组(P=0.034).单因素Cox回归分析进一步显示,SCARNA4高表达与患者的不良预后显著相关(HR=2.285,95%CI:1.040~5.020,P=0.039).多因素Cox回归分析证实,在调整相关协变量后,SCARNA4表达水平是影响肺腺癌患者总生存期的独立危险因素,其高表达与患者总生存期缩短显著相关(HR=3.038,95%CI:1.261~7.323,P=0.013).结论 SCARNA4在肺腺癌组织中表达上调,与患者不良预后相关,可能通过调控增殖、迁移和侵袭等方式促进肿瘤进展,有望成为肺腺癌治疗的新靶点和预后生物标志物.
Objective To analyze the differential expression profiles of small nucleolar RNAs(snoRNAs)in lung adenocarcinoma and their association with prognosis,screen and validate lung adenocarcinoma-related snoRNAs,and explore their roles in tumorigenesis and progression.Methods Differentially expressed snoRNAs between lung adenocarcinoma and normal tissues were screened using Arraystar Small RNA expression microarrays.The obtained candidates were validated through the GEO database(GSE261702),followed by selecting snoRNAs that passed molecular cloning experiments,and finally RT-qPCR.By constructing SCARNA4 overexpression models(Vector group and SCARNA4 group)and knockdown models(siNC group and si SCARNA4 group),proliferation,migration and invasion assays were carried out to assess the biological functions of SCARNA4 in lung adenocarcinoma cells.Based on tumor tissues from 108 lung adenocarcinoma patients(Second Affiliated Hospital of Army Medical University,between February 2013 and May 2015),the expression level of SCARNA4 was detected by RT-qPCR.Using X-tile software to determine the optimal cut-off value(3.48),the patients were accordingly stratified into high(57 cases)and low SCARNA4 expression(51 cases)groups.Kaplan-Meier survival curves and Cox proportional hazards regression models were constructed to analyze the impact of SCARNA4 expression on prognosis.Results Small RNA microarray identified 62 up-regulated and 4 down-regulated snoRNAs in lung adenocarcinoma tissues.Integration with GEO database and molecular cloning yielded 8 candidate snoRNAs.RT-qPCR results revealed significantly elevated SCARNA4 expression in lung adenocarcinoma tissues than normal tissues(P=0.042 7).Overexpression of SCARNA4 significantly promoted the proliferative,migrative,and invasive capacities in A549 cells(P<0.01),whereas its knockdown obviously inhibited these functions(P<0.01).Kaplan-Meier survival analysis demonstrated significantly shorter overall survival in the high-expression group when compared with the low-expression group(P=0.034).Univariate Cox regression analysis further confirmed that high SCARNA4 expression was significantly associated with poor prognosis(HR=2.285,95%CI:1.040 to 5.020,P=0.039).Multivariate Cox regression analysis confirmed that,after adjusting for relevant covariates,the expression level of SCARNA4 was an independent risk factor of overall survival of lung adenocarcinoma patients,and its high expression was notably associated with shortened overall survival of patients(HR=3.038,95%CI:1.261 to 7.323,P=0.013).Conclusion SCARNA4 is up-regulated in lung adenocarcinoma tissues and associated with poor prognosis.It may be involved in the tumorigenesis and development of lung adenocarcinoma by regulating cell proliferation,migration,and invasion.The molecule might hold promise as a novel therapeutic target and prognostic biomarker for lung adenocarcinoma.
彭青云;白莉;杨敬源;李亚斐;谢薇佳;夏婷婷;单亦凡;向颖;邬娜;李成英;吴龙;余祖滨
贵州医科大学公共卫生与健康学院,环境污染与疾病监控教育部重点实验室,贵州贵阳||陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)第二附属医院:全军呼吸内科研究所,全军呼吸病研究重点实验室,重庆贵州医科大学公共卫生与健康学院,环境污染与疾病监控教育部重点实验室,贵州贵阳陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)军事预防医学系军队流行病学教研室,重庆陆军军医大学(第三军医大学)第二附属医院:胸外科,重庆
医药卫生
小核仁RNASCARNA4肺腺癌致癌作用预后
small nucleolar RNASCARNA4adenocarcinoma of lungcarcinogenesisprognosis
《陆军军医大学学报》 2026 (5)
572-582,11
国家自然科学基金面上项目(82372652)陆军军医大学红医苗圃人才项目(2022) Supported by the General Program of National Natural Science Foundation of China(82372652)and the Red Medical Nursery Talent Program of Army Medical University(2022).
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