微小RNA-203b-3p调控多发性骨髓瘤细胞增殖、迁移和侵袭的分子机制研究

目的 观察微小RNA-203b-3p(miR-203b-3p)通过调节肿瘤坏死因子超家族成员13b(TNFSF13B)对多发性骨髓瘤(MM)细胞的影响,探讨miR-203b-3p抑制MM的相关机制。方法 采用实时荧光定量聚合酶链式反应(qRT-PCR)和蛋白质印迹分析(Western blot)检测miR-203b-3p和TNFSF13B在骨髓瘤肿瘤和细胞中的表达情况。miR-203b-3p与TNFSF13B的关系采用双荧光素酶报告实验进行验证。Lipofectamine 2000试剂用于MM细胞转染。miR-203b-3p和TNFSF13B对MM细胞生物功能的影响采用克隆形成试验、划痕试验和Transwell试验进行分析。结果 与癌旁组织及正常细胞比较,MM组织和细胞中miR-203b-3p的表达量相对较低,而TNFSF13B在MM肿瘤和细胞中的表达量与正常组织和细胞相比升高,差异有统计学意义(P<0.05)。双荧光素酶报告实验结果表明,TNFSF13B是miR-203b-3p的直接靶点。miR-203b-3p在MM细胞中的过量表达能够抑制细胞的增殖和转移,差异有统计学意义(P<0.05),而TNFSF13B的表达上调则促进了MM细胞的增殖、迁移和侵袭,差异有统计学意义(P<0.05)。结论 miR-203b-3p可能通过下调TNFSF13B抑制MM细胞的增殖、侵袭和转移。

microRNA-199a/b-3p对乳腺癌细胞运动能力的影响

目的:探讨microRNA-199a/b-3p抑制乳腺癌细胞运动能力的机制。方法:在乳腺癌MDA-MB-231细胞中,转入miR-199a/b-3p mimcs,免疫印迹法检测PAK4的表达量变化;迁移和侵袭实验检测,超表达miR-199a/b-3p和干扰PAK4表达对乳腺癌迁移侵袭的影响;细胞膜皱起检测,超表达miR-199a/b-3p和干扰PAK4表达对乳腺癌细胞细胞膜皱起的影响。结果:在MDA-MB-231细胞中,超表达miR-199a/b-3p或干涉内源PAK4蛋白表达,均能下调细胞的迁移率、侵袭率和平均细胞膜皱起面积。结论:miR-199a/b-3p抑制乳腺癌细胞运动能力部分是通过抑制PAK4表达实现的,且miR-199a/b-3p具有抗乳腺癌迁移药物开发的潜质。

microRNA-199a/b-3p表达与肝细胞癌临床预后的相关性

目的:检测肝癌组织中micro RNA-199a/b-3p的表达变化,探讨mi R-199a/b-3p表达与肝细胞癌临床预后的相关性。方法:通过荧光定量检测法检测肿瘤组织与相应癌旁组织中mi R-199a/b-3p的表达变化,分析其与临床病例参数的相关性。结果:肝细胞癌患者肿瘤组织中mi R-199a/b-3p表达水平较癌旁组织均显著下调(P<0.05);发生转移患者的肝癌组织中mi R-199a/b-3p表达低于未转移患者;mi R-199a/b-3p高表达肝细胞癌患者的无瘤生存时间优于低表达患者(P<0.05)。结论:mi R-199a/b-3p低表达可能与肝细胞癌转移及预后不良相关。

MicroRNA-199a/b-3p抑制三阴乳腺癌细胞增殖机制研究

目的:探讨microRNA-199a/b-3p(miR199)抑制三阴乳腺癌细胞增殖存活的作用机制。方法:在三阴乳腺癌细胞BT549、MDA-MB-231转染miR199,荧光定量检测miR199表达量;MTT法检测转染miR199对三阴乳腺癌细胞存活率的影响;细胞周期分析检测,转染miR199对在乳腺癌细胞细胞周期的影响。结果:超表达miR199后,三阴乳腺癌细胞BT549、MDA-MB-231的增殖率分别下降(41.02±2.34)%和(28.42±6.70)%,细胞周期均被阻滞在G1期。结论:miR-199a/b-3p抑制三阴乳腺癌增殖,具有抗三阴乳腺癌增殖药物开发的潜质。

肝细胞癌患者血清microRNA-92b-3p的表达及其意义

目的探讨肝细胞癌(HCC)患者血清microRNA-92b-3p的表达水平及其辅助诊断的价值。方法选择79例HCC、40例肝硬化(LC)患者以及40例健康对照者为研究对象,对3组血清标本中的microRNA-92b-3p、甲胎蛋白(AFP)和维生素K缺乏诱导蛋白(PIVKA-Ⅱ)水平进行了检测。结果 HCC患者血清microRNA-92b-3p相对表达量显著高于LC组和健康组,差异均有统计学意义(P<0.05);而LC组与健康组microRNA-92b-3p比较差异无统计学意义(P=0.135)。HCC患者血清microRNA-92b-3p相对表达量在血管浸润、TNM分期、LC相关分组间差异有统计学意义(P<0.05)。HCC患者血清microRNA-92b-3p相对表达量与AFP(R2=0.041,P=0.073)、PIVKA-Ⅱ(R2=0.083,P=0.011)无相关性。microRNA-92b-3p、AFP、PIVKA-Ⅱ3项联合检测诊断HCC时的曲线下面积为0.941,灵敏度为93.67%,诊断效能最佳。结论 HCC患者血清microRNA-92b-3p水平升高,检测microRNA-92b-3p水平对HCC具有一定的辅助诊断价值,可能成为HCC诊断中的重要生物学指标之一。

早期肝细胞癌患者循环microRNA-199a/b-3p的检测及临床意义

目的:检测早期肝细胞癌患者血清中microRNA-199a/b-3p的表达变化,探讨在肝细胞癌诊断中的价值。方法:收集肝细胞癌患者血清标本30例、肝硬化患者血清标本30例、健康人血清标本30例。提取血清总RNA逆转录,应用荧光定量检测法检测血清中miRNA-199a/b-3p的表达变化,并与AFP进行比较。结果:肝细胞癌、肝硬化患者血清miRNA-199a/b-3p水平均显著低于健康对照组(P<0.05);miRNA-199a/b-3p诊断肝硬化和早期肝细胞癌的准确度及阳性率均优于AFP。结论:血清miRNA-199a/b-3p表达变化对早期肝细胞癌和肝硬化的具有一定的诊断价值。

Effect of miR-27b-3p and Nrf2 in human retinal pigment epithelial cell induced by high-glucose

AIM:To determine whether the microRNA-27b-3p(miR-27b-3p)/NF-E2-related factor 2(Nrf2)pathway plays a role in human retinal pigment epithelial(hRPE)cell response to high glucose,how miR-27b-3p and Nrf2 expression are regulated,and whether this pathway could be specifically targeted.METHODS:hRPE cells were cultured in normal glucose or high glucose for 1,3,or 6d before measuring cellular proliferation rates using cell counting kit-8 and reactive oxygen species(ROS)levels using a dihydroethidium kit.miR-27b-3p,Nrf2,NAD(P)H quinone oxidoreductase 1(NQO1)and heme oxygenase-1(HO-1)mRNA and protein levels were analyzed using reverse transcription quantitative polymerase chain reaction(RT-qPCR)and immunocytofluorescence(ICF),respectively.Western blot analyses were performed to determine nuclear and total Nrf2 protein levels.Nrf2,NQO1,and HO-1 expression levels by RT-qPCR,ICF,or Western blot were further tested after miR-27b-3p overexpression or inhibitor lentiviral transfection.Finally,the expression level of those target genes was analyzed after treating hRPE cells with pyridoxamine.RESULTS:Persistent exposure to high glucose gradually suppressed hRPE Nrf2,NQO1,and HO-1 mRNA and protein levels and increased miR-27b-3p mRNA levels.High glucose also promoted ROS release and inhibited cellular proliferation.Nrf2,NQO1,and HO-1 mRNA levels decreased after miR-27b-3p overexpression and,conversely,both mRNA and protein levels increased after expressing a miR-27b-3p inhibitor.After treating hRPE cells exposed to high glucose with pyridoxamine,ROS levels tended to decreased,proliferation rate increased,Nrf2,NQO1,and HO-1 mRNA and protein levels were upregulated,and miR-27b-3p mRNA levels were suppressed.CONCLUSION:Nrf2 is a downstream target of miR-27b-3p.Furthermore,the miR-27b-3p inhibitor pyridoxamine can alleviate high glucose injury by regulating the miR-27b-3p/Nrf2 axis.

MicroRNA-15b-3p对三阴性乳腺癌细胞增殖、迁移能力的影响

目的 研究MicroRNA-15b-3p对HCC1937三阴性乳腺癌细胞株增殖、迁移、凋亡能力的影响。方法 选用乳腺癌细胞株MCF-7、T47D、HCC1937及MDA-MB-468作为研究模型,实时荧光定量PCR方法分别检测4种细胞株中hsa-miR-15b-3p的表达情况。体外培养HCC1937细胞,将上调后的MicroRNA-15b-3p转染至HCC1937细胞株中设为实验组,并设置阴性对照组,Brdu实验检测细胞乳腺癌细胞的增殖能力、Transwell小室检测细胞迁移能力、FACS细胞凋亡检测细胞凋亡情况。结果 hsa-miR-15b-3p在不同的乳腺癌细胞株中表达量均较正常乳腺细胞少,实验组细胞增殖能力强于阴性对照组(P<0.05),实验组乳腺癌细胞的迁移能力强于阴性对照组(P<0.05),但实验组与对照组细胞凋亡水平差异无显著性。结论 MicroRNA-15b-3p可增强三阴性乳腺癌细胞的增殖、迁移能力,有可能会促进乳腺癌的发生与发展。

miR-148b-3p对施万细胞增殖的影响

目的 :探讨microRNA-148b-3p(miR-148b-3p)对施万(Schwann)细胞增殖的影响及作用的靶基因。方法 :采用Edu染色法检测miR-148b-3p对原代培养的施万细胞增殖能力的影响;基因芯片及生物信息学分析筛选miR-148b-3p可能作用的靶基因;实时定量PCR检测施万细胞中过表达miR-148b-3p模拟物后靶基因的表达变化。结果 :miR-148b-3p能明显促进原代培养的施万细胞的增殖,miR-148b-3p过表达可抑制其靶基因Alcam、Cpd、Dedd、Nptx2、Phf20、Ptpn14和Stard 13的表达。结论 :miR-148b-3p有可能通过对增殖相关靶基因的负调控来影响施万细胞的增殖能力,从而促进周围神经损伤修复。

miR-92b-3p靶向肌细胞增强子2D抑制心肌细胞肥大

【目的】探讨微小RNAmicroRNA-92b-3p(mi R-92b-3p)对心肌细胞肥大的调控作用及其作用靶基因。【方法】建立血管紧张素Ⅱ(Ang-Ⅱ)诱导的C57BL/6小鼠心肌肥厚模型。通过尾静脉注射胆固醇修饰的mi R-92b-3p模拟物(agomi R-92b-3p)来增加小鼠心肌中mi R-92b-3p水平,分别设立3个实验组:agomi R-negative control(agomi R-NC)+saline组,agomi RNC+Ang-Ⅱ组,agomi R-92b-3p+Ang-Ⅱ组。用Ang-Ⅱ诱导乳小鼠心肌细胞建立心肌细胞肥大模型;双荧光素酶报告基因实验检测mi R-92b-3p与潜在靶基因MEF2D 3'端非翻译区(3'-UTR)的结合作用;蛋白印迹法检测MEF2D及肥厚相关蛋白的表达。【结果】(1)Ang-II诱导的小鼠肥厚心肌和肥大心肌细胞分别与对照组中心肌肥厚相关基因ANP、ACTA1和β-MHC水平比较,差异具有统计学意义(P<0.05);(2)双荧光素酶报告基因实验结果提示mi R-92b-3p与MEF2D 3′UTR具有相互结合作用;mi R-92b-3p可在转录后水平抑制MEF2D的表达;升高mi R-92b-3p或降低MEF2D水平能一致性地抑制Ang-II诱导的乳小鼠心肌细胞肥大表型。【结论】MEF2D是mi R-92b-3p的靶基因,并介导了mi R-92b-3p发挥抑制心肌细胞肥大的作用。

OXT通过miR-196b-3p/ASPP2信号通路调节卵巢癌细胞生长

目的探讨催产素(oxytocin,OXT)对卵巢癌细胞增殖与凋亡的影响及其作用机制。方法人卵巢癌细胞系SKOV3和A2780细胞来源于美国模式培养物保藏所(ATCC)。OXT和OXT受体(oxytocin receptor,OXTR)拮抗剂Atosiban刺激卵巢癌细胞,改变细胞中miR-196b-3p的水平,使用MTT法、ELISA试验、Western blot、生物信息学工具及荧光素酶报告基因实验等研究以上处理对卵巢癌细胞增殖与凋亡的作用和机制。结果OXT刺激SKOV3细胞OXTR激活(F=28.842,P<0.05),增殖活性降低(F=12.988,P<0.05),Caspase3活性增加(F=26.676,P<0.05);Ki67、增殖细胞核抗原(proliferating cell nuclear antigen,PCNA)及p53凋亡刺激蛋白抑制剂(inhibitor of apoptosis-stimulating of p53 protein,iASPP)表达下调,p53凋亡刺激蛋白(apoptosis-stimulating of p53 protein,ASPP)1(ASPP1)及2(ASPP2)表达上调;但Atosiban部分逆转OXT的效果。OXT刺激卵巢癌细胞miR-196b-3p水平减少(A2780:F=76.406,P<0.05;SKOV3:F=45.874,P<0.05)。miR-196b-3p-mimic转染联合OXT刺激,导致细胞增殖活性增加(F=9.232,P<0.05),Caspase3活性降低(F=36.350,P<0.05),同时ASPP2表达降低(F=83.013,P<0.05)。而miR-196b-3p-inhibitor转染联合OXT刺激,ASPP2表达增加(F=83.013,P<0.05)。生物信息学工具预测联合荧光素酶报告基因实验确认ASPP2是miR-196b-3p的靶基因。结论OXT介导的OXTR激活通过调节miR-196b-3p/ASPP2信号通路调节卵巢癌细胞生长。

Lnc-MEG3调控miR-10b-5p/CD82轴对垂体瘤细胞增殖、侵袭的影响

目的探究lnc-MEG3对垂体瘤细胞增殖、侵袭的调控机制。方法取垂体瘤HP75细胞分为对照组、si-NC组、si-MEG3组、pcDNA3.1-NC组、oe-MEG3组、oe-MEG3+mimic-NC组、oe-MEG3+miR-10b-5p mimic组。转染后,检测细胞中lnc-MEG3、miR-10b-5p和CD82 mRNA的表达水平、细胞增殖、迁移、侵袭能力和细胞中CD82、PCNA、E-cadherin、N-cadherin、MMP-9蛋白表达。结果Lnc-MEG3过表达可降低miR-10b-5p,上调CD82和E-cadherin水平,降低PCNA、N-cadherin、MMP-9水平,抑制垂体瘤细胞增殖、迁移和侵袭(P<0.05);上调miR-10b-5p可抑制CD82,减弱lnc-MEG3过表达对垂体瘤细胞增殖、侵袭和迁移的抑制作用。双荧光素酶报告基因检测结果显示,转染miR-10b-5p mimic后,细胞中MEG3-WT和CD82-WT的荧光素酶活性显著降低(P<0.05)。结论Lnc-MEG3过表达可能通过靶向下调miR-10b-5p,进而上调CD82的表达,抑制垂体瘤细胞增殖、迁移和侵袭。

Long noncoding RNA X-inactive specific transcript regulates NLR family pyrin domain containing 3/caspase-1-mediated pyroptosis in diabetic nephropathy

BACKGROUND NLRP3-mediated pyroptosis is recognized as an essential modulator of renal disease pathology.Long noncoding RNAs(lncRNAs)are active participators of diabetic nephropathy(DN).X inactive specific transcript(XIST)expression has been reported to be elevated in the serum of DN patients.AIM To evaluate the mechanism of lncRNA XIST in renal tubular epithelial cell(RTEC)pyroptosis in DN.METHODS A DN rat model was established through streptozotocin injection,and XIST was knocked down by tail vein injection of the lentivirus LV sh-XIST.Renal metabolic and biochemical indices were detected,and pathological changes in the renal tissue were assessed.The expression of indicators related to inflammation and pyroptosis was also detected.High glucose(HG)was used to treat HK2 cells,and cell viability and lactate dehydrogenase(LDH)activity were detected after silencing XIST.The subcellular localization and downstream mechanism of XIST were investigated.Finally,a rescue experiment was carried out to verify that XIST regulates NLR family pyrin domain containing 3(NLRP3)/caspase-1-mediated RTEC pyroptosis through the microRNA-15-5p(miR-15b-5p)/Toll-like receptor 4(TLR4)axis.RESULTS XIST was highly expressed in the DN models.XIST silencing improved renal metabolism and biochemical indices and mitigated renal injury.The expression of inflammation and pyroptosis indicators was significantly increased in DN rats and HG-treated HK2 cells;cell viability was decreased and LDH activity was increased after HGtreatment. Silencing XIST inhibited RTEC pyroptosis by inhibiting NLRP3/caspase-1. Mechanistically,XIST sponged miR-15b-5p to regulate TLR4. Silencing XIST inhibited TLR4 by promotingmiR-15b-5p. miR-15b-5p inhibition or TLR4 overexpression averted the inhibitory effect ofsilencing XIST on HG-induced RTEC pyroptosis.CONCLUSIONSilencing XIST inhibits TLR4 by upregulating miR-15b-5p and ultimately inhibits renal injury inDN by inhibiting NLRP3/caspase-1-mediated RTEC pyroptosis.

干扰PAK4表达对肝细胞癌迁移侵袭的影响

目的:探讨利用microRNA-199a/b-3p干扰PAK4表达抑制肝细胞癌迁移侵袭的机制。方法:在HEK293T细胞中转入miR-199a/b-3p mimcs和pmir GLO-PAK4 3'UTR,荧光素酶报告法检测miR-199a/b-3p对PAK4的抑制作用。在肝细胞癌SMMC-7721细胞中,转入miR-199a/b-3p mimcs,免疫印迹法检测PAK4的表达量变化;迁移和侵袭实验检测,miR-199a/b-3p对肝细胞癌迁移侵袭的影响,干扰PAK4表达后肝细胞癌迁移侵袭的影响。结果:在SMMC-7721细胞中,miR-199a/b-3p通过与PAK4 3'UTR结合抑制PAK4 mRNA翻译,导致PAK4表达降低,并通过抑制PAK4表达抑制肝细胞癌迁移侵袭。结论:miR-199a/b-3p能抑制肝细胞癌细胞迁移侵袭,具有抗肝细胞癌药物开发的潜质。

microRNA-203a-3p在原发性肝癌患者外周血中的临床研究

目的对不同分期原发性肝癌患者外周血中microRNA-203a-3p表达进行荧光定量PCR检测,研究microRNA-203a-3p在原发性肝癌患者中的临床意义。方法收集56例原发性肝癌患者外周血,另取56例同期健康者作为对照组并留取血样。荧光定量PCR实验测定血样microRNA-203a-3p表达水平。与健康者相比,统计microRNA-203a-3p在不同分期原发性肝癌患者的表达水平,并分析与AFP数值的相关性以及15例肝癌患者治疗前后microRNA-203a-3p的差异。结果与健康者相比,56例原发性肝癌患者外周血中microRNA-203a-3p显著降低,和原发性肝癌分期相关,与AFP水平显著负相关,且15例原发性肝癌手术患者治疗1个月后microRNA-203a-3p表达显著升高,差异有统计学意义(P<0.05)。结论MicroRNA-203a-3p在原发性肝癌患者外周血中显著降低并和临床进程显著相关。

慢病毒介导MicroRNA-376b-3p对垂体腺瘤细胞增殖和凋亡的影响及机制探究

目的:探究慢病毒介导MicroRNA-376b-3p对垂体腺瘤增殖和凋亡的影响及其可能的机制。方法:以体外培养的人垂体腺瘤细胞系为研究对象,分别设立为MicroRNA-376b-3p mimics组(对照组)和慢病毒lenti-sh MicroRNA-376b-3p组(药物组),采用MTT法检测MicroRNA-376b-3p对垂体腺瘤细胞增殖的影响,AnnexinV-FITC/PI双染法检测MicroRNA-376b-3p对垂体腺瘤细胞凋亡率的影响,Western blot法检测MicroRNA-376b-3p对高迁移率蛋白A2(HMGA2)、Bcl-2相关X蛋白(Bax)、半胱氨酸天冬氨酸蛋白酶-3(Caspase-3)蛋白表达的影响。结果:(1)慢病毒介导MicroRNA-376b-3p能够显著抑制垂体腺瘤细胞的增殖(P<0.05);(2)在MicroRNA-376b-3p干预后12 h、24 h以及48 h,垂体腺细胞的凋亡率均明显升高(P<0.05);(3)经MicroRNA-376b-3p转染后,Bax蛋白表达升高,Bcl-2、Caspase-3、Survivin以及HMGA2蛋白表达降低(P<0.05)。结论:慢病毒介导MicroRNA-376b-3p能够明显抑制垂体腺瘤细胞增殖,诱导其凋亡,分析其作用机制可能与下调HMGA2和Survivin表达及上调Bax蛋白表达有关。

miR-296抑制自噬促进角膜新生血管生成

目的本研究探讨miR-296在角膜新生血管生成中的作用以及其对自噬蛋白LC3B-Ⅰ/Ⅱ、P62的调控作用。方法利用血管内皮生长因子诱导人脐静脉内皮细胞(HUVECs)建立体外角膜新生血管模型。实验分为6组(Control组、模型组、VEGF+miR-296 mimic NC组、VEGF+miR-296 mimic组、VEGF+miR-296 inhibitor NC组、VEGF+miR-296 inhibitor组)。采用RT-qPCR检测miR-296在体外新生血管中的表达;转染过表达或者低表达miR-296,采用CCK-8、划痕实验、成管实验探究miR-296在体外角膜新生血管生成中的作用;采用KEGG和GO分析预测miR-296参与的通路及其靶基因的作用;采用Western blot检测miR-296对自噬蛋白LC3B-Ⅰ/Ⅱ、P62表达的影响。结果RT-qPCR结果显示,与Control组相比,模型组中miR-296表达升高[(2.84±0.23)比(1.32±0.04),t=6.42,P<0.01];与VEGF+miR-296 mimic NC组相比,VEGF+miR-296 mimic组细胞的吸光度[(1.24±0.02)比(1.07±0.01),t=7.55,P<0.05]、迁移数[(123.30±2.60)比(85.33±2.33),t=10.87,P<0.01]、分支数[(128.70±2.73)比(107.30±1.20),t=7.16,P<0.05]升高;与VEGF+miR-296 inhibitor NC组相比,VEGF+miR-296 inhibitor组细胞的吸光度[(0.82±0.01)比(1.06±0.02),t=11.69,P<0.05]、迁移数[(62.00±1.16)比(84.33±1.8),t=10.59,P<0.01]、分支数[(85.67±2.60)比(102.30±1.45),t=5.59,P<0.05]降低;KEGG和GO分析预测了miR-296及其靶基因可能参与血管生成类通路和自噬水平的调控;western blot显示,与VEGF+miR-296 mimic NC组相比,VEGF+miR-296 mimic组细胞中LC3B-Ⅱ蛋白表达降低[(1.27±0.05)比(1.57±0.05),t=4.46,P<0.05],p62蛋白表达升高[(1.30±0.02)比(0.85±0.04),t=10.91,P<0.01];相反,与VEGF+miR-296 inhibitor NC组相比,VEGF+miR-296 inhibitor组细胞中LC3B-Ⅱ蛋白表达升高[(2.37±0.01)比(0.04±0.03),t=11.78,P<0.01],p62蛋白表达降低[(0.52±0.02)比(0.85±0.03),t=9.24,P<0.01]。结论miR-296在体外可促进角膜新生血管生成,且此过程与自噬水平的下调有关。

LncRNA AFAP1-AS1/miR-27b-3p/VEGF-C axis modulates stemness characteristics in cervical cancer cells

Background:Long non-coding RNA(lncRNA)actin filament-associated protein 1 antisense RNA 1(AFAP1-AS1)functions as a competing endogenous RNA to regulate target genes expression by sponging microRNAs(miRs)to play cancer-promoting roles in cancer stem cells.However,the regulatory mechanism of AFAP1-AS1 in cervical cancer(CC)stem cells is unknown.The present study aimed to provide a new therapeutic target for the clinical treatment of CC.Methods:Hyaluronic acid receptor cluster of differentiation 44 variant exon 6(CD44v6)(+)CC cells were isolated by flow cytometry(FCM).Small interfering RNAs of AFAP1-AS1(siAFAP1-AS1)were transfected into the(CD44v6)(+)cells.The levels of AFAP1-AS1 were measured by quantitative real-time PCR(qRT-PCR).Sphere formation assay,cell cycle analysis,and Western blotting were used to detect the effect of siAFAP1-AS1.RNA pull-down and luciferase reporter assay were used to verify the relationship between miR-27b-3p and AFAP1-AS1 or vascular endothelial growth factor(VEGF)-C.Results:CD44v6(+)CCcells had remarkable stemness and a high level ofAFAP1-AS1.However,AFAP1-AS1knockdownwithsiAFAP1-AS1suppressed the cell cycle transitionofG(1)/S phase and inhibited self-renewal ofCD44v6(+)CCcells,the levels of the stemnessmarkers octamer-binding transcription factor 4(OCT4),osteopontin(OPN),and cluster of differentiation 133(CD133),and the epithelialmesenchymal transition(EMT)-related proteins Twist1,matrix metalloprotease(MMP)-9,and VEGF-C.In the mechanism study,miR-27b-3p/VEGF-C signaling was demonstrated to be a key downstream of AFAP1-AS1 in the CD44v6(+)CC cells.Conclusions:LncRNA AFAP1-AS1 knockdown inhibits the CC cell stemness by upregulating miR-27b-3p to suppress VEGF-C.