Expression of MTA2 Gene in Ovarian Epithelial Cancer and Its Clinical Implication

In order to investigate the roles of MTA2 in the pathogenesis of ovarian epithelial cancer, the expression of MTA2 in 4 ovarian cell lines were detected by semi-quantitative RT-PCR and Western-blot assays. MTA2 expression in normal, borderline, benign and malignant epithelial ovarian tissues was immunohistochemically examined. The expression of MTA2 mRNA and protein was detected in all of 4 cell lines of ovarian epithelial cancer. The expression of MTA2 mRNA and protein was higher in strong migration cell lines than in weak migration ones. In borderline and ma lignant ovarian tissues tested, MTA2 staining was dramatically stronger than in normal and benign tissues （P〈0. 01）. The expression levels in malignant ovarian tissues were significantly higher than that in borderline epithelial ovarian tissues （P〈0.01）. The expression of MTA2 was correlated with clinical stage, histopathological grade and lymph node metastasis. It was concluded that the high expression of MTA2 was associated with more aggressive behaviors of epithelial ovarian cancer. MTA2 provides a novel indicator of ovarian cancer.

Expression of Bmi-1 and EZH2 in tissues adjacent to human epithelial ovarian cancer cells of orthotopic implantation in nude mice

Objective This study investigated the feasibility of screening residual normal ovarian tissues based on the expression of Bmi-1 and EZH2 in tissues adjacent to orthotopic ovarian carcinomas in nude mice. Methods The human epithelial ovarian cancer cell line OVCAR3 was grown in subcutaneous tissues and the tumor tissues were orthotopically implanted. The expression levels of Bmi-1 and EZH2 were detected by immunohistochemical staining and RT-PCR in cancer tissues, proximal and remote tissues with respect to the cancer tissues, and normal ovarian tissues of nude mice.Results Thirty-five ovarian tissue samples with normal biopsy results were obtained from 40 cases of human epithelial ovarian cancer in the nude mice in which the tumor tissues were orthotopically implanted. Bmi-1 and EZH2 expression levels were lower in proximal paraneoplastic tissue samples than in cancer tissue samples(P < 0.05) and higher than in remote paraneoplastic tissue samples(P < 0.01). No significant difference was found in the expression levels of Bmi-1 and EZH2 using immunohistochemistry among residual normal ovarian tissues obtained from orthotopically implanted models that differed in severity. The expression of Bmi-1 and EZH2 was negative in 20 normal ovarian tissue samples.Conclusion The expression levels of Bmi-1 and EZH2 were reduced with increasing distance from the cancer tissues. Negative expression of these tumor-associated genes can be used as a standard for the screening of normal ovarian tissues adjacent to tumor tissues. Normal ovarian tissues can be obtained from the tissues adjacent to tumors.

Establishment of an optimized CTC detection model consisting of EpCAM,MUC1 and WT1 in epithelial ovarian cancer and its correlation with clinical characteristics

Objective:Emerging studies have demonstrated the promising clinical value of circulating tumor cells(CTCs)for diagnosis,disease assessment,treatment monitoring and prognosis in epithelial ovarian cancer.However,the clinical application of CTC remains restricted due to diverse detection techniques with variable sensitivity and specificity and a lack of common standards.Methods:We enrolled 160 patients with epithelial ovarian cancer as the experimental group,and 90 patients including 50 patients with benign ovarian tumor and 40 healthy females as the control group.We enriched CTCs with immunomagnetic beads targeting two epithelial cell surface antigens(EpCAM and MUC1),and used multiple reverse transcription-polymerase chain reaction(RT-PCR)detecting three markers(EpCAM,MUC1 and WT1)for quantification.And then we used a binary logistic regression analysis and focused on EpCAM,MUC1 and WT1 to establish an optimized CTC detection model.Results:The sensitivity and specificity of the optimized model is 79.4%and 92.2%,respectively.The specificity of the CTC detection model is significantly higher than CA125(92.2%vs.82.2%,P=0.044),and the detection rate of CTCs was higher than the positive rate of CA125(74.5%vs.58.2%,P=0.069)in early-stage patients(stage I and II).The detection rate of CTCs was significantly higher in patients with ascitic volume≥500 mL,suboptimal cytoreductive surgery and elevated serum CA125 level after 2 courses of chemotherapy(P<0.05).The detection rate of CTC;and CTC;was significantly higher in chemo-resistant patients(26.3%vs.11.9%;26.4%vs.13.4%,P<0.05).The median progression-free survival time for CTC;patients trended to be longer than CTC;patients,and overall survival was shorter in CTC;patients(P=0.043).Conclusions:Our study presents an optimized detection model for CTCs,which consists of the expression levels of three markers(EpCAM,MUC1 and WT1).In comparison with CA125,our model has high specificity and demonstrates better diagnostic values,especially for early-stage ovarian cancer.Detection of CTC;and CTC;had predictive value for chemotherapy resistance,and the detection of CTC;suggested poor prognosis.

IDENTIFICATION OF DIFFERENTIAL GENES IN OVARIAN CANCER USING REPRESENTATIONAL DIFFERENCE ANALYSIS OF cDNA

Objoctive To identify differential genes between normal ovarian epithelium tissue and ovarian epithelial cancer using representational difference analysis of cDNA （cDNA-RDA）. Methods cDNA-RDA was performed to identify the differentially expressed sequences between cDNAs from cancer tissue and cDNAs from normal ovarian tissue in the same patient who was in the early stage of ovarian serous cystadenocarcinoma. These differentially expressed fragments were cloned and analyzed, then sequenced and compared with known genes. Results Three differentially cxpressed cDNA fragments were isolated using cDNA from normal ovarian tissue as tester and cDNA from cancer tissue as driver amplicon by cDNA-RDA. DP Ⅲ- 1 and DP Ⅲ-2 cDNA clone showed significant homology to the cDNA of alpha actin gene; DPⅢ-3 cDNA clone showed significant homology to the cDNA oftransgelin gene. Conclusion cDNA-RDA can bc used to sensitively identify the differentially expressed genes in ovarian serous cystadenocarcinoma. Ovarian serous cystadenocarcinoma involves alteration of multiple genes.

PAX8基因与上皮性卵巢癌的相关性

上皮性卵巢癌由几种不同的组织学亚型构成,其中最常见的是高级别浆液性卵巢癌,约占侵袭性上皮性卵巢癌的70%。近年研究发现该疾病可能源自输卵管分泌上皮。配对盒基因PAX8是谱系特异的转录因子相关基因,在输卵管正常发育过程中发挥重要作用,同时可通过多种途径参与上皮性卵巢癌的发生。越来越多研究者认为PAX8基因与肿瘤细胞迁移、侵袭、增殖、细胞存活、干细胞维持相关,但其在卵巢癌中的具体作用机制仍不明确。因此,研究PAX8基因在上皮性卵巢癌中表达的特点及作用机制,可能为该型卵巢癌寻找有效的肿瘤标志物,进而为卵巢癌的诊断、预后及治疗等提供新思路。

影像组学列线图在卵巢肿瘤诊断中的应用

卵巢肿瘤病理类型繁多,异质性明显。影像学检查为诊断卵巢肿瘤提供了可靠的依据。影像组学在传统影像学技术的基础上,高通量地提取及分析特征,已被用于卵巢肿瘤的诊断、分期、预后分析等方面。列线图模型通过整合多方面的预测因素,量化具体临床事件的风险,被广泛应用于肿瘤学研究。本文就国内外基于影像组学的列线图模型应用于卵巢肿瘤诊断中的研究作一综述,并探讨该技术所面临的挑战及发展前景。

Rank sum method for related gene selection and its application to tumor diagnosis

Tumor diagnosis by analyzing gene expression profiles becomes an interesting topic in bioinformatics and the main problem is to identify the genes related to a tumor. This paper proposes a rank sum method to identify the re- lated genes based on the rank sum test theory in statistics. The tumor diagnosis system is constructed by the support vector machine (SVM) trained on the set of the related gene expression profiles. The experiments demonstrate that the constructed tumor diagnosis system with the rank sum method and SVM can reach an accuracy level of 96.2% on the colon data and 100% on the leukemia data.

MRI联合血清TSGF、NDRG4在上皮性卵巢癌诊断中的作用

目的探讨血清肿瘤特异性生长因子(TSGF)、N-Myc下游调节基因4(NDRG4)在上皮性卵巢癌血清中的表达以及联合磁共振成像(MRI)在上皮性卵巢癌诊断中的作用。方法收集本院2021年1月~2022年8月期间进行手术的60例上皮性卵巢癌患者(卵巢癌组)作为研究对象,同时选取与上皮性卵巢癌患者临床资料一致的妇科良性肿瘤患者(良性组)和健康体检者(对照组)各60例。比较各组血清TSGF、NDRG4水平;ROC曲线分析血清TSGF、NDRG4分别对上皮性卵巢癌的诊断效能;四表格法分析MRI联合血清TSGF、NDRG4对上皮性卵巢癌的诊断效能。结果卵巢癌组血清TSGF水平显著高于良性组和对照组(P<0.05),血清NDRG4水平显著低于良性组和对照组(P<0.05);良性组血清TSGF水平显著高于对照组(P<0.05),血清NDRG4水平显著低于对照组(P<0.05)。MRI联合血清TSGF、NDRG4诊断上皮性卵巢癌的准确率为93.33%,敏感性为95.00%,特异性为91.67%。其中,三项联合诊断的特异性高于NDRG4、MRI单独诊断(P<0.05),三项联合诊断的准确率和敏感性高于TSGF、NDRG4单独诊断(P<0.05)。结论上皮性卵巢癌患者血清TSGF的表达水平显著升高,NDRG4的表达水平显著降低,MRI联合血清TSGF、NDRG4对上皮性卵巢癌具有一定的诊断价值。

卵巢癌转移耐药相关基因的全基因组表达序列分析

目的利用Agilent全基因组寡核苷酸基因表达谱芯片探寻与卵巢癌转移和耐药相关的基因表达序列,初步探讨卵巢癌转移耐药相关的分子机制。方法通过全基因组基因芯片检测高转移性及耐药性的上皮性卵巢癌细胞系RMG-1-H、COC1/DDP和HO8910/PM与其各自对应的RMG-1-C、COC1和HO8910细胞系基因表达序列,探寻差异表达的基因并对其进行基因本体论分析、通路分析及交互作用网络分析,并用实时PCR和免疫组织化学方法验证芯片结果。结果有49个基因发生2倍以上的表达差异,主要涉及基因表达、生物聚合物的合成等方面,交互网络图预测出对相互作用发挥连接作用的21个基因。采用实时聚合酶链反应及免疫组织化学方法对差异表达基因GCET2、CFTR、FOXP1和GARS在细胞和组织中进行基因及蛋白水平验证,结果与芯片结果相一致。结论与卵巢癌转移和化疗耐药相关的基因表达谱序列的变化可以为卵巢癌转移和化疗耐药的相关分子机制研究提供理论基础。

半边旗提取物5F对人高转移卵巢癌细胞HO-8910PMETS-1mRNA和VEGF蛋白表达的影响

目的:研究半边旗提取物5F(以下简称5F)对HO-8910PM细胞内VEGF蛋白及ETS-1mRNA表达的影响,探讨其抗肿瘤侵袭转移的作用机制.方法:RT-PCR分析ETS-1mRNA的表达;Western blot分析VEGF蛋白的表达.结果:25～100 μmol/L 5F作用HO-8910PM细胞24 h后,明显下调ETS-1mRNA的表达;5F明显下调VEGF蛋白表达水平.结论:5F抗肿瘤侵袭转移能力与ETS-1mRNA和VEGF蛋白的表达有关.

KAI1/CD82和E-Cadherin蛋白在卵巢上皮性癌中表达的临床意义

目的:探讨肿瘤转移抑制基因KAI1和粘附分子钙粘蛋白基因E-Cadherin的表达与卵巢上皮性癌临床病理因素的相关性。方法:对66例肿瘤标本应用免疫组织化学SP法检测KAI1/CD82和E-Cadherin蛋白在卵巢上皮性癌组织中的表达,生物学统计采用χ2检验法。结果:KAI1/CD82蛋白表达的阳性率为57.58%(38/66);E-Cadherin蛋白阳性率为46.97%(31/66)。两种基因蛋白表达与肿瘤临床分期及淋巴结转移密切相关,差异有统计学意义(P<0.05);KAI1/CD82蛋白的表达与肿瘤的组织学分级呈负相关(P<0.05)。在同一标本中,二者表达有较好的相关性和一致性,差异具有统计学意义(P<0.05)。结论:KAI1/CD82和E-Cadherin蛋白的表达与卵巢上皮性癌的演进和转移密切相关,检测其表达异常对判断肿瘤的分化、临床进展以及推测预后有一定的参考价值。

卵巢癌组织中Vasohibin基因表达与启动子区域甲基化的关系

目的探讨卵巢上皮性肿瘤中Vaso-hibin基因mRNA表达与临床特征及其启动子甲基化的关系。方法用RT-PCR检测10例良性卵巢上皮性肿瘤、8例交界性卵巢上皮性肿瘤及30例卵巢癌组织中VasohibinmRNA表达;用甲基化特异聚合酶链反应方法(MSP)检测Vasohibin启动子甲基化。结果各组标本中都有VasohibinmRNA表达,3组Vasohib-in表达的相对值良性卵巢上皮性肿瘤为0.65±0.11,交界性卵巢上皮性肿瘤为0.47±0.13,卵巢癌为0.34±0.14。卵巢癌组织中Vasohibin的表达量较交界性卵巢上皮性肿瘤组织显著降低,t=2.479,P=0.029;交界性卵巢上皮性肿瘤组织的表达量较良性卵巢上皮性肿瘤显著下降,t=3.198,P=0.006。在卵巢癌组织中,Vasohibin的表达与不同临床分期、不同分化程度以及有无淋巴结转移无关。良性卵巢上皮性肿瘤中未发现Vasohibin基因启动子甲基化;交界性卵巢上皮性肿瘤中2例发生启动子甲基化,卵巢癌中11例发生启动子甲基化,甲基化率36.7%。卵巢癌中启动子甲基化组织较未甲基化组织VasohibinmRNA表达显著降低,t=4.671,P=0.000。结论Vasohibin与卵巢癌发生存在明显相关性。Vasohibin启动子甲基化与其mRNA表达抑制密切相关,可能是Vasohibin在卵巢癌中低表达的最主要因素之一。

上皮性卵巢癌组织中FOXC1 mRNA表达变化及其启动子区甲基化情况观察

目的观察卵巢上皮性肿瘤中FOXC1 mRNA表达变化及其启动子区甲基化情况。方法选择30例上皮性卵巢癌(A组)、14例交界性卵巢上皮性肿瘤(B组)和21例良性卵巢上皮性肿瘤患者(C组),取其手术切除卵巢组织标本,用RT-PCR法检测FOXC1 mRNA,用甲基化特异聚合酶链反应方法(MSP)结合琼脂糖凝胶电泳检测FOXC1基因启动子区甲基化状态及频率。结果 A、B、C组FOXC1 mRNA相对表达量分别为0.38±0.16、0.61±0.18、1.19±0.17,A组低于B组,B组低于C组(P均<0.05)。A组卵巢癌组织中FOXC1 mRNA相对表达量与临床分期及分化程度无关,与淋巴结转移有关(P<0.05)。A、B、C组卵巢组织中FOXC1基因启动子区甲基化频率分别为66.7%、50.0%、9.5%,A组高于B组,B组高于C组(P均<0.05)。A组FOXC1基因启动子区甲基化、未甲基化者FOXC1 mRNA相对表达量分别为0.32±0.14、0.45±0.17,P<0.05。结论上皮性卵巢癌组织中FOXC1 mRNA表达下降,FOXC1 mRNA表达与上皮性卵巢癌淋巴结转移有关。FOXC启动子区甲基化状态与其mRNA表达抑制相关。

NDRG4通过Wnt/β-catenin信号转导通路抑制卵巢癌细胞的迁移和侵袭能力

目的探讨N-myc downstream regulated gene 4(NDRG4)对卵巢癌SKOV3细胞迁移和侵袭能力的影响及其分子机制。方法应用脂质体转染法将NDRG4过表达载体pcDNA3.1-NDRG4质粒(pcDNA3.1-NDRG4质粒组)和空白pcDNA3.1质粒(空白质粒组)转染至SKOV3细胞中。采用实时荧光定量PCR和Western blot法验证NDRG4过表达效果,应用transwell小室法检测细胞迁移和侵袭能力的变化,Western blot法检测卵巢癌细胞中上皮间质转化相关蛋白(E-cadherin、N-cadherin和Vimentin)以及Wnt/β-catenin信号通路相关蛋白(β-catenin和c-myc)的表达水平。结果转染48 h后,与空白质粒组比较,pcDNA3.1-NDRG4质粒组细胞迁移和侵袭能力均下降(P=0.006,P=0.023)。转染72 h后,与空白质粒组比较,pcDNA3.1-NDRG4质粒组E-cadherin表达水平上升(P=0.023),N-cadherin和Vimentin的表达水平均下降(P=0.013,P=0.021)。转染72 h后,与空白质粒组比较,pcDNA3.1-NDRG4质粒组β-catenin和c-myc的表达水平均下降(P=0.035,P=0.006)。结论NDRG4蛋白抑制卵巢癌细胞迁移和侵袭能力,并抑制上皮间质转化过程。该作用可能是通过抑制Wnt/β-catenin细胞信号通路实现。

ZNF191 mRNA在卵巢恶性肿瘤中的表达及临床意义

采用RT-PCR方法检测31例卵巢恶性肿瘤组织和31例正常卵巢组织中ZNF191 mRNA的表达。结果显示,与正常卵巢组织相比,ZNF191 mRNA在卵巢恶性肿瘤组织中的表达显著下调(P<0.01);在浆液性癌、黏液性癌、宫内膜样癌等上皮性卵巢癌中的下调程度显著大于颗粒细胞瘤(P<0.05).而在上皮性卵巢癌各组织类型间无显著差异;ZNF191 mRNA的表达水平在不同分期、不同分化程度的卵巢恶性肿瘤中无显著差异。本组资料提示ZNF191基因的变异参与了卵巢恶性肿瘤的发生,可能在卵巢恶性肿瘤的早期发病机制中发挥作用,。

中国人卵巢上皮性肿瘤nm23H1基因遗传不稳定性的研究

采用石蜡包埋组织抽提DNA,PCR-单链构象多态性(PCR-SSCP),常规银染、Envision免疫组织化学染色和Leica-Qwin计算机图像分析等方法,研究人类17号染色体D17S396位点微卫星不稳定(microsatellite instablility,MSI)和杂合性缺失(loss of heterozygosity,LOH),对卵巢上皮性肿瘤nm23H1蛋白表达的影响,阐明nm23H1基因遗传不稳定性与卵巢肿瘤进展的关系,为揭示nm23H1基因作用机制和肿瘤转移机制提供实验依据。本实验中,卵巢上皮性癌D17S396位点遗传不稳定发生率为40%,明显高于交界性肿瘤的9.52%,而在良性肿瘤和正常卵巢组织中,未见该位点遗传不稳定的发生。其中,LOH的发生率,随肿瘤恶性程度的增高而增加(P<0.05)。在卵巢上皮性癌中,淋巴转移组的LOH发生率高于无淋巴转移组(P<0.01)。FIGO Ⅲ+Ⅳ期的LOH发生率高于Ⅰ+Ⅱ期(P<0.05)。MSI发生率与卵巢上皮癌组织类型、分化程度、淋巴转移及FIGO分期均无关。nm23H1 蛋白阳性率在卵巢上皮性癌和交界性肿瘤组织中分别为56.00%和57.14%,高于良性肿瘤的13.64%和正常卵巢组织的8.33%(P<0.01)。卵巢上皮性癌中,淋巴转移组nm23H1蛋白阳性率低于无淋巴转移组;FIGO Ⅲ+Ⅳ期nm23H1蛋白阳性率低于Ⅰ+Ⅱ期(P<0.05)。此外,计算机图像定量分析显示,在各临床病理参数影响下,nm23H1蛋白的表达强度没有差异。在卵巢上皮性癌中,LOH阳性组中nm23H1蛋白阳性率为0.00%,显著低于LOH阴性组的73.68%(P<0.01)。实验结果提示, nm23H1基因的遗传不稳定性可能是卵巢上皮性癌发生、发展的一个重要机制。LOH的发生可作为卵巢组织恶变的判断指标。nm23H1基因的MSI和LOH,通过相互独立的途径调控卵巢上皮癌的发生和转移,后者可抑制卵巢上皮癌局部nm23H1蛋白的表达,并赋予卵巢上皮癌高淋巴结转移、低预后的特性。提高卵巢上皮癌局部nm23H1蛋白的表达,可减缓肿瘤的淋巴转移并提高预后率。

CA125、CA153、CA199和CEA联合检测在上皮性卵巢癌中的诊断价值

目的探讨血清中CA125、CA153、CA199和CEA四项肿瘤标志物的联合检测在上皮性卵巢癌诊断中的价值。方法采用化学发光免疫测定法检测54例卵巢癌患者和68例卵巢良性病变患者手术前,以及55例对照组(无妇科疾病及恶性疾病)妇女的血清样本中CA125、CA153、CA199及CEA水平。应用统计软件SPSS 13.0和MedCalc 10.4.0.0回顾性分析检测结果。结果计算每种标志物单项及联合检测的敏感度、特异度及准确度。CA125三项指标分别为96.3%、64.7%和78.7%,高于其他单项指标。而联合检测中CA125联合CA153敏感度高达99.1%,准确度为79.5%,分别高于单项最佳的CA125及其他联合检测方式(P<0.05)。结论使用CA125与CA153联合检测对上皮性卵巢癌的诊断价值优于CA125单项检测及其他组合方式。

转染人附睾蛋白4基因对人卵巢癌细胞基因表达的影响

目的探讨转染人附睾蛋白4(HE4)基因对卵巢癌细胞ES-2基因表达的影响。方法构建HE4高表达及空质粒对照组细胞系,通过基因芯片探寻存在差异表达的基因,并对其进行基因本体(GO)注释和富集分析、京都基因与基因组百科全书(KEGG)通路分析,并对芯片结果进行验证。结果有639个基因发生了差异表达,其中上调基因283个,下调基因356,实时PCR及免疫组化方法对差异表达基因FOXA2和SERPIND1进行了RNA和蛋白水平的验证,结果与芯片结果相一致。GO富集分析发现差异基因在生物过程中,参与了生物高聚物代谢、程序性细胞死亡及凋亡等,KEGG通路分析发现这些基因与MAPK、性激素生物合成、癌症、细胞周期和p53信号等有关。结论与HE4相关的基因表达谱序列的变化可以为HE4在卵巢癌中功能及作用通路等分子机制的研究提供理论基础。

铂类耐药相关基因在卵巢癌顺铂耐药形成过程中表达量的动态变化

目的了解卵巢癌患者在铂类治疗过程中产生获得性耐药相关基因表达动态变化的情况,为临床预后的预测及个体化治疗奠定理论基础。方法采用Benjamini-Hochberg(BH)法对源于TCGA数据库(The Cancer Genome Atlas)的256例敏感和耐药患者的卵巢癌全基因表达谱数据进行差异表达基因筛选。采用DAVID软件中的KEGG模块对筛选出的差异基因进行通路富集,筛选出P<0.05的通路,对筛选出的通路所包含的基因采用成组t检验找出差异显著的基因(P<0.05)。对筛选出的基因采用COREMINE工具进行文本挖掘,找出与多药耐药及肿瘤耐药存在线性相关的基因,将其与患者预后进行分析,确定存在差异显著的基因。采用实时荧光定量PCR法检测所筛选出的基因在裸鼠诱导耐药模型不同给药阶段的表达变化情况。结果 BH法共筛选出306个差异表达基因,其中上调基因110个,下调基因196个。DAVID软件的KEGG模块分别筛选出5条上调及4条下调通路,成组t检验筛选出有差异的基因共37个,其中上调基因18个,下调基因19个。COREMINE工具检索出与多药耐药及肿瘤耐药存在线性相关的上调基因为ITPA、IMPDH2、RPS7、PDE5A和PDE4D,下调基因为GNAS、CFTR、BUB3、PRKDC、RBL2、SMC1A、CALR、CCNE2及CHEK1。生存分析结果提示CALR及PRKDC基因的表达与患者生存时间有关,CALR和PRKDC基因高表达组的患者生存时间长于低表达组。qRT-PCR检测发现,CALR和PRKDC基因随顺铂注射次数增多,在SKOV3-GFP及SKOV3/DDPⅱ肿瘤组织中的表达量逐渐降低。结论 CALR与PRKDC基因可能与卵巢癌铂类耐药及患者的预后密切相关,且随着耐药的产生,CALR和PRKDC基因的表达量逐渐降低。

lncRNA在肿瘤中的表达及作用机制

长链非编码RNA(long non-coding RNAs,lncRNAs)是一类转录本长度大于200 nt,不具有蛋白编码功能的非编码RNA.近年来,随着高通量测序技术的发展,越来越多的功能性lncRNAs逐渐被发现,且已成为研究的热点.研究发现,lncRNAs可以作为致癌或抑癌基因参与肿瘤的发生发展.通过比对肿瘤细胞和正常细胞的表达谱显示,多种lncRNAs在不同类型肿瘤中异常表达.除了表型上的研究,目前已有部分报道深入研究了lncRNAs在肿瘤中的作用机制.例如,lncRNAs与肿瘤细胞凋亡、转移及耐药等过程密切相关.此外,在肿瘤患者的临床常规检验中检测到lncRNAs,提示其能够作为一种潜在的肿瘤诊断和预后因子.lncRNAs有望成为新型肿瘤标志物和肿瘤治疗的靶点,用于诊断、治疗、预测预后.本文将通过对lncRNAs在肿瘤中的作用及其分子机制进行综述.