Therapeutic Effect of Bone Marrow Mesenchymal Stem Cells on Rat Bladder Cancer

Objective:To analyze the effect of bone marrow mesenchymal stem cell therapy on rats with bladder cancer and provide a feasible direction for the treatment of human bladder cancer.Methods:An animal model was constructed,and Model 1 was used as an example.Two groups of rats were injected with anti-upconversion nanoparticles(UCNPs)(experimental group)and 0.9%normal saline(control group),respectively.In vivo imaging was performed to determine the accuracy of the anti-UCNPs method.Results:There were 15 rats in the experimental group with obvious bladder swelling.Among them,11 rats had cauliflower-like and partially brown bladder tumors,whereas the other four rats had hard,nodular-like protrusions,with indistinct borders and adhesions to the anterior wall of the rectum.Small papillary masses were observed in two rats,local mucosal thickening without tumor formation was observed in two rats,and bladder stones were observed in six rats.The bladder specimens of 15 rats in the control group were pink and shiny,without any tumors.Fourteen rats in the experimental group and 12 rats in the control group had bladder cancer lesions,accounting for 93.33%and 80%,respectively.The detection accuracy of the experimental group was significantly better than that of the control group.Conclusion:Multimodal nanoprobes targeting bladder cancer stem cells in vivo were used to image the orthotopic tumor and lymph node metastasis models of animals by anti-UCNPs imaging to observe the distribution,migration,and differentiation process of bladder cancer stem cells in model mice.It is clear that rare earth upconversion luminescent nanomaterials,modified by BCMab1 and CD44 monoclonal antibodies,can be used as probes for the detection of bladder cancer,the tracking of lymph node metastasis in bladder cancer,and the comprehensive evaluation of the overall efficacy of nanoprobe-targeted therapy for bladder cancer stem cells.

Research Progress of Prostate Stem Cell Antigen in Bladder Cancer Treatment

In order to study the application effect of prostate stem cell antigen in the treatment of bladder cancer,several literatures have been reviewed in this paper,including the predisposition factors of bladder cancer,clinical treatment methods,progress of prostate stem cell antigen,and nanomaterial probe.This paper presents a feasible method of using luminescent nanomaterials(anti-UCNPs)as biological probes.

Molecular Assessment of Non-Muscle Invasive and Muscle Invasive Bladder Tumors: Mapping of Putative Urothelial Stem Cells and Toll-Like Receptors (TLR) Signaling

Purpose: The main objectives of this study were to characterize and compare the urothelial stem cells (healthy and cancer cells) and TLRs features in the urinary bladder of men without lesionsand with non-muscle-invasive and muscle invasive urothelial tumors. Materials and Methods: Thirty samples of the urinary bladder of 50 to 80-year-old men, with and without diagnosis of malignant urothelial lesions were used. The 30 samples were divided into 3 groups (n = 10 per group): Normal Group;Non-Muscle Invasive Bladder Cancer Group;Muscle Invasive Bladder Cancer Group. The samples were histopathologically and immunohistochemically analyzed. The study was conducted at teaching Hospital of the University of Campinas (UNICAMP). Results: The CD44 and CD133 immunoreactivities were significantly intense in the muscle-invasive cancer group when compared to the other groups. The ABCG2 biomarker demonstrated intense immunoreactivities in both non-muscle and muscle invasive groups, and absent immunoreactivity in the normal group. All groups showed weak CD117 immunoreactivity. Putative Healthy Stem Cells (CD44/CD133/ CD117+) occurred in all groups. Putative Cancer Stem Cells (CD44/CD133/ABCG2+) only occurred in the non-muscle and muscle invasive cancer groups. TLR2 immunoreactivity was significantly lower in the non-muscle invasive cancer group and absent in the muscle invasive cancer group. TLR4 immunoreactivity was significantly lower in both cancer groups. Conclusions: This study leads us to the conclusion that putative cancer stem cell occurrence was sensitive to the decreased in TLR2 and TLR4 immunoreactivities. Also, TLR2 and TLR4 demonstrated their involvement in the regulation of the different biomarkers for putative healthy and cancer urothelial stem cells, probably acting as negative regulators of urothelial carcinogenesis. Taken together data obtained suggest that use of TLRs agonists could be a promising alternative for the treatment of non-muscle and muscle invasive bladder tumors.

Stem cell applications for pathologies of the urinary bladder

New stem cell based therapies are undergoing intense research and are widely investigated in clinical fields including the urinary system. The urinary bladder performs critical complex functions that rely on its highly coordinated anatomical composition and multiplex of regulatory mechanisms. Bladder pathologies resulting in severe dysfunction are common clinical encounter and often cause significant impairment of patient's quality of life. Current surgical and medical interventions to correct urinary dysfunction or to replace an absent or defective bladder are sub-optimal and are associated with notable complications. As a result, stem cell based therapies for the urinary bladder are hoped to offer new venues that could make up for limitations of existing therapies. In this article, we review research efforts that describe the use of different types of stem cells in bladder reconstruction, urinary incontinence and retention disorders. In particular, stress urinary incontinence has been a popular target for stem cell based therapies in reported clinical trials. Furthermore, we discuss the relevance of the cancer stem cell hypothesis to the development of bladder cancer. A key subject that should not be overlooked is the safety and quality of stem cell based therapies introduced to human subjects either in a research or a clinical context.

Expression and Significance of Oct4 in Bladder Cancer

In order to detect the expression of Oct4 in bladder cancer tissue and cell line BIU-87, immunohistochemistry was used in 49 bladder cancer biopsy samples and immunofluorescence and reverse transcription-PCR were performed on bladder cancer cell line BIU-87. Forty of 49 bladder cancer samples showed the expression of Oct4 in about 0.6% cancer cells, The positive rate and density of Oct4 expression had no obvious relationship with the grade, recurrence or metastasis of bladder cancer （P〉0.05）. A few Oct4 positive cells were found in bladder cancer cell line BIU-87, which was also confirmed by RT-PCR. This study indicated the existence of few Oct4 positive cells in bladder cancer, which may be the bladder cancer stem cells. This study may provide the foundation for isolation and identification of bladder cancer stem cells.

长链非编码RNA在膀胱癌干细胞中的研究现状及展望

膀胱癌是泌尿系统常见恶性肿瘤之一,具有高发病率和死亡率,且治疗后易出现复发和转移。越来越多的证据表明,具有启动和维持肿瘤生长的肿瘤干细胞是膀胱癌治疗失败的主要原因,所以,靶向膀胱癌干细胞的治疗方式成为了目前研究重点。研究发现长链非编码RNA(lncRNA)是膀胱癌干细胞的关键调节因子,多种lncRNA参与癌症干性。这些lncRNA可以调节干细胞相关转录因子在膀胱癌中的表达。其在膀胱癌的发生和进展中发挥重要作用,目前已经被研究为抗癌治疗的靶标。为此本文对不同lncRNA在分子水平上如何调控膀胱癌干细胞特性进行综述,为未来膀胱癌的临床治疗提供理论依据及可行方向。

WNT/β-catenin signaling in urothelial carcinoma of bladder

Urothelial carcinoma of bladder is the second most prevalent genitourinary disease.It is a highly heterogeneous disease as it represents a spectrum of neoplasms,including non-muscle invasive bladder cancer(NMIBC),muscle invasive bladder cancer(MIBC)and metastatic lesions.Genome-wide approaches and candidate gene analysis suggest that malignant transformation of the bladder is multifactorial and a multitude of genes are involved in the development of MIBC or NMIBC phenotypes.Wnt signaling is being examined to control and maintain balance between stemness and differentiation in adult stem cell niches.Owing to its participation in urothelial development and maintenance of adult urothelial tissue homeostasis,the components of Wnt signaling are reported as an important diagnostic and prognostic markers as well as novel therapeutic targets.Mutations/epigenetic alterations in the key molecules of Wnt/β-catenin canonical pathway have been linked with tumorigenesis,development of drug resistance and enhanced survival.Present review extends our understanding on the functions of key regulatory molecules of canonical Wnt/β-catenin pathway in urothelial tumorigenesis by inducing cancer stem cell phenotype(UCSCs).UCSCs may be responsible for tumor heterogeneity,high recurrence rates and complex biological behavior of bladder cancer.Therefore,understanding the role of UCSCs and the regulatory mechanisms that are responsible for high relapse rates and metastasis could help to develop pathway inhibitors and augment current therapies.Potential implications in the treatment of urothelial carcinoma of bladder by targeting this pathway primarily in UCSCs as well as in bulk tumor population that are responsible for high relapse rates and metastasis may facilitate potential therapeutic avenues and better prognosis.

lncRNA NNT-AS1对膀胱癌细胞增殖、转移及肿瘤干细胞干性的影响与机制研究

目的探究长链非编码RNA(lncRNA)NNT-AS1对膀胱癌细胞增殖、转移及肿瘤干细胞干性的影响和机制。方法qRT-PCR检测lncRNA NNT-AS1在膀胱癌细胞T24、5637、UM-UC-3、TCC-SUP和膀胱上皮细胞SV-HUC-1中的表达,将T24细胞和膀胱癌干细胞分为sh-NC组(转染sh-NC)、sh-NNT-AS1组(转染sh-NNT-AS1)、Control组(共转染sh-NC、inh-NC和si-NC)、sh-NNT-AS1+inh-NC+si-NC组(共转染sh-NNT-AS1、inh-NC和si-NC)、sh-NNT-AS1+inh-582-5p+si-NC组(共转染sh-NNT-AS1、miR-582-5p抑制物和si-NC)、sh-NNT-AS1+inh-582-5p+si-NCKAP1组(共转染sh-NNT-AS1、miR-582-5p抑制物和NCKAP1小干扰RNA)。CCK8检测各组细胞增殖能力;Transwell法检测细胞迁移和侵袭能力;细胞成球实验检测各组干细胞干性;流式细胞术检测CD133和CD44表达;双荧光素酶报告基因实验检测lncRNA NNT-AS1与miR-582-5p及miR-582-5p与NCKAP1的靶向关系;体内成瘤实验检测lncRNA NNT-AS1对体内成瘤的影响;Western blot检测NCKAP1、YAP、TAZ、CD44、ALDH1A1、Oct4、Nanog蛋白表达。结果lncRNA NNT-AS1高表达于T24、5637、UM-UC-3、TCC-SUP细胞。与sh-NC组比较,sh-NNT-AS1组T24细胞增殖、迁移和侵袭能力显著下降(P<0.05),膀胱癌干细胞成球数、CD44、ALDH1A1、Oct4、Nanog蛋白表达及CD133^(+)CD44^(+)细胞比例显著减少(P<0.05)。lncRNA NNT-AS1调控miR-582-5p/NCKAP1分子轴。与Control组比较,sh-NNT-AS1+inh-NC+si-NC组细胞光密度(OD)值显著降低(P<0.05),细胞迁移和侵袭数显著减少(P<0.05),膀胱癌干细胞干性显著降低(P<0.05),肿瘤体积显著减小(P<0.05),YAP和TAZ表达显著下调(P<0.05)。与sh-NNT-AS1+inh-NC+si-NC组比较,sh-NNT-AS1+inh-582-5p+si-NC组细胞OD值、细胞迁移数和侵袭数均显著升高/增加(P<0.05),膀胱癌干细胞干性、肿瘤体积显著增加(P<0.05),YAP和TAZ表达均显著升高(P<0.05)。与sh-NNT-AS1+inh-582-5p+si-NC组比较,sh-NNT-AS1+inh-582-5p+si-NCKAP1组细胞OD值、细胞迁移数和侵袭数均显著降低/减少(P<0.05),膀胱癌干细胞干性、肿瘤体积显著减小(P<0.05),YAP和TAZ表达均显著降低(P<0.05)。结论lncRNA NNT-AS1通过调控miR-582-5p/NCKAP1分子轴影响膀胱癌细胞的增殖、转移及肿瘤干细胞干性,并激活Hippo-YAP/TAZ信号通路。

P300/CBP相关因子在BCa细胞DNA损伤修复与肿瘤干细胞干性维持中的作用

目的探究P300/CBP相关因子(PCAF)在人膀胱癌(BCa)细胞DNA损伤修复与肿瘤干细胞干性维持中的作用。方法利用Ad-PCAF RNAi转染人膀胱癌细胞系5637,荧光显微镜和Western blot检测转染效果,选择顺铂诱导膀胱癌细胞DNA损伤,MTS法检测损伤细胞的增殖活性,免疫荧光染色检测损伤细胞内PCAF与γ-H2AX的募集情况,细胞彗星实验分析顺铂诱导细胞DNA损伤的程度;从膀胱癌细胞中分选CD44^(+)标记的肿瘤干细胞,Western blot检测Bca干细胞标志物67LR、OCT4及YAP1蛋白表达水平变化,细胞成球实验检测细胞干性变化。结果Ad-PCAF RNAi转染5637细胞后,明显抑制了细胞中PCAF表达(P<0.05);在下调PCAF表达后,20、40、60、80、100 nmol/L的顺铂处理下5637细胞活性下降,增强了5637细胞对顺铂的敏感性,细胞内γ-H2AX焦点形成明显增加,细胞拖尾较长,拖尾细胞数目和尾距均增加(P<0.05);经分选得到CD44^(+)比例为93%且67LR、OCT4及YAP1蛋白呈阳性表达的膀胱癌干细胞,通过下调PCAF表达,肿瘤干细胞的球体体积变小,成球个数也减少(P<0.05)。结论通过下调PCAF的表达能够抑制膀胱癌细胞DNA损伤修复,调控肿瘤干细胞的干性维持。

LncRNANNT-AS1通过调控miR-582-5p/NCKAP1轴激活Hippo-YAP/TAZ信号通路促进膀胱癌细胞增殖、迁移、侵袭和干细胞干性影响

目的检测膀胱癌中长链非编码RNA(long non-coding RNA,lncRNA)烟酰胺核苷酸转氢酶反义RNA1(nicotinamide nucleotide transhydrogenase antisense RNA 1,NNT-AS1)表达情况,研究其对膀胱癌细胞增殖、迁移、侵袭及肿瘤干细胞干性的影响及可能分子机制。方法实时荧光定量PCR(quantitative real-time PCR,qRT-PCR)法检测膀胱癌组织标本及细胞中LncRNA NNT-AS1表达情况;将膀胱癌细胞转染分为sh-NC组,sh-NNT-AS1组,sh-NNT-AS1+inh-582-5p组和sh-NNT-AS1+inh-582-5p+si-NCKAP1组。采用CCK-8法检测细胞增殖吸光度值(A值);Transwell实验检测细胞迁移、侵袭穿膜数;细胞成球实验检测干细胞干性。检索starBase和TargetScan数据库,并通过双荧光素酶报告基因实验预测验证LncRNA NNT-AS1和miR-582-5p,miR-582-5p与NCKAP1的靶向结合关系。Western blot检测膀胱癌干细胞标志蛋白(CD44,ALDH1A1,Oct4,Nanog)及Hippo-YAP/TAZ信号通路相关蛋白表达灰度值。结果与癌旁组织相比,膀胱癌组织中LncRNA NNT-AS1表达水平(0.34±0.07 vs 1.15±0.21)明显升高,差异有统计学意义(t=16.364,P<0.001)。与人正常膀胱上皮SV-HUC-1细胞(1.00±0.01)相比,膀胱癌细胞T24,5637,UM-UC-3和TCC-SUP中LncRNA NNT-AS1表达(6.03±0.17,4.66±0.36,5.47±0.26,3.02±0.20)明显升高,差异有统计学意义(t=17.472~51.160,均P<0.001)。与sh-NC组相比,在24,48和72 h时sh-NNT-AS1组细胞增值能力(A值)均显著降低(0.80±0.01 vs 1.07±0.06,1.18±0..07 vs 1.83±0.03,1.89±0.07 vs 2.53±0.06),差异有统计学意义(t=7.688,14.783,12.024,均P<0.05);sh-NNT-AS1组细胞迁移穿膜数(55.00±2.65个vs 354.30±7.84个)、细胞侵袭穿膜数(45.67±2.33个vs 303.00±9.07个)及膀胱癌干细胞成球数(20.85±2.17个vs 41.35±3.67个)显著降低,差异具有统计学意义(t=-62.641,-47.596,8.328,均P<0.001)。与sh-NC组相比,sh-NNT-AS1组细胞中CD44(0.04±0.01 vs 1.12±0.02),ALDH1A1(0.23±0.01 vs 1.16±0.05),Oct4(0.17±0.02 vs 1.10±0.04),Nanog(0.49±0.03 vs 1.24±0.03)的蛋白表达灰度值显著降低,差异具有统计学意义(t=83.656,31.591,36.019,30.619,均P<0.001)。与si-NC组相比,sh-NNT-AS1组CD44+CD133+细胞比例(9.30%±0.79%vs 88.50%±2.77%)明显降低,差异有统计学意义(t=-47.624,P<0.001)。双荧光素酶报告基因检测结果显示miR-582-5p为LncRNANNT-AS1靶基因,NCKAP1为miR-582-5p靶基因;LncRNA NNT-AS1靶向调控miR-582-5p/NCKAP1轴。与sh-NNT-AS1组相比,在24,48,72 h时sh-NNT-AS1+inh-582-5p组细胞增值能力(A值)均明显升高(0.98±0.03 vs 0.73±0.06,1.74±0.04 vs 1.22±0.05,2.33±0.16 vs 1.69±0.14),差异有统计学意义(t=5.977~11.628,均P<0.001)。与sh-NNT-AS1+inh-582-5p组相比,在24,48,72 h时sh-NNT-AS1+inh-582-5p+si-NCKAP1组细胞增值能力(A值)显著降低(0.69±0.04,1.01±0.07,1.39±0.08),差异有统计学意义(t=7.877~16.323,均P<0.001)。与sh-NNT-AS1组相比,sh-NNT-AS1+inh-582-5p组细胞迁移穿膜数(322.31±28.45个vs 81.42±13.22个)、细胞侵袭穿膜数(316.07±30.21个vs 92.13±12.65个)及膀胱癌干细胞成球数(38.55±2.20个vs 18.98±1.16个)显著增加,差异具有统计学意义(t=15.115,13.158,14.592,均P<0.001)。与sh-NNT-AS1组相比,sh-NNT-AS1+inh-582-5p组细胞CD44(1.05±0.08 vs 0.10±0.01),ALDH1A1(1.20±0.16 vs 0.22±0.02),Oct4(1.32±0.14 vs 0.19±0.03),Nanog(0.97±0.12 vs 0.15±0.04),YAP(1.29±0.11 vs 0.42±0.07)和TAZ(1.41±0.16 vs 0.35±0.05)蛋白表达灰度值均显著增加,差异具有统计学意义(t=10.650~21.243,均P<0.001)。与sh-NNT-AS1+inh-582-5p组相比,sh-NNT-AS1+inh-582-5p+si-NCKAP1组细胞迁移穿膜数(65.33±12.60个)、细胞侵袭穿膜数(71.08±15.19个)、膀胱癌干细胞成球数(11.36±1.05个)均显著降低,差异具有统计学意义(t=16.125,14.395,21.365,均P<0.001)。与sh-NNT-AS1+inh-582-5p组相比,sh-NNT-AS1+inh-582-5p+si-NCKAP1组细胞CD44(0.25±0.05),ALDH1A1(0.61±0.11),Oct4(0.22±0.08),Nanog(0.44±0.07),YAP(0.25±0.09)和TAZ(0.30±0.04)蛋白表达灰度值显著降低,差异具有统计学意义(t=6.412~17.889,均P<0.001)。结论膀胱癌中LncRNA NNT-AS1表达上调,其对膀胱癌细胞增殖、侵袭及肿瘤干细胞干性的影响,可能是通过调控miR-582-5p/NCKAP1分子轴,激活Hippo-YAP/TAZ信号通路完成。

肿瘤干细胞标记物ALDH1在非浸润性膀胱癌组织中的表达及其临床意义

目的:探讨肿瘤干细胞标记物乙醛脱氢酶1(ALDH1)在非浸润性膀胱癌组织中的表达,初步了解肿瘤干细胞与膀胱癌生物学特征的关系。方法:采用免疫组织化学法检测118例非浸润性膀胱癌组织及30例癌旁正常膀胱组织中ALDH1的表达,并结合临床病理及预后资料进行关联性分析。结果:在非浸润性膀胱癌组织中ALDH1阳性表达率为24.58%,在癌旁正常膀胱组织中为6.67%,2组比较差异有统计学意义(P<0.05);在低级别和高级别非浸润性膀胱癌组织中ALDH1阳性表达率分别为18.18%(14/77)和36.59%(15/41),二者比较差异有统计学意义(P<0.05);在pTa期和pT1期非浸润性膀胱癌组织中ALDH1阳性表达率分别为16.92%(11/65)和33.96%(18/53),二者比较差异有统计学意义(P<0.05);在初发和复发的非浸润性膀胱癌组织中ALDH1阳性表达率分别为19.77%(17/86)和37.50%(12/32),差异有统计学意义(P<0.05);ALDH1表达与非浸润性膀胱癌患者性别、年龄及肿瘤大小无明显关联性(P>0.05)。术后随访4～52个月,ALDH1阳性表达组和阴性表达组无瘤生存率分别为55.17%和61.80%,Kaplan-Merier曲线及Log-rank检验,2组患者累积无瘤生存时间比较差异有统计学意义(P<0.05)。结论:ALDH1表达与膀胱癌病理分级、分期及肿瘤复发有关联。肿瘤干细胞可能在非浸润性膀胱癌的发生和复发中具有重要作用。

人膀胱癌组织中肿瘤干细胞样细胞的分离培养及PIWIL2表达

目的从人膀胱移行细胞癌(BTCC)组织中分离培养肿瘤干细胞样细胞(CSLC),鉴定其生物学特性,并研究PIWIL2在CSLC中的表达和意义。方法收集12例不同临床分期BTCC患者组织标本,通过酶消化和原代培养相结合等方法处理,采用无血清悬浮培养法分离培养获得含CSLC的悬浮细胞球,流式细胞仪检测细胞表面分子标志CD133和CD44的表达,免疫磁珠分选系统分离CD133+CD44+细胞;采用半定量逆转录聚合酶链反应检测PIWIL2mRNA在CSLC中的表达;裸鼠皮下接种CS-LC,观察其成瘤能力。结果成功地从人膀胱癌组织分离培养获得可悬浮生长、稳定传代的CSLC,CSLC高表达CD133和CD44,裸鼠皮下接种1×104、1×105个CSLC均可全部成瘤,PIWIL2mRNA在CSLC的表达显著高于正常膀胱组织细胞。结论采用无血清悬浮培养法成功从人膀胱癌组织中分离获得CSLC,具有肿瘤干细胞特性,能高度表达PIWIL2,为靶向肿瘤干细胞的治疗提供了实验依据。

肿瘤干细胞标记蛋白ALDH1在浸润性膀胱癌组织中的表达及其与临床病理和预后的关系

目的：探讨肿瘤干细胞标记物乙醛脱氢酶1（ALDH1）在浸润性膀胱癌组织中的表达,阐明其与膀胱癌生物学行为的关系。方法：采用免疫组织化学方法检测109例浸润性膀胱癌组织和20例癌旁正常膀胱组织（对照组）中ALDH1蛋白的表达,同时检测6例癌转移淋巴结组织及20例未转移淋巴结组织中ALDH1的表达,分析ALDH1蛋白表达与浸润性膀胱癌患者临床病理特征的关系及其对患者总生存率和无瘤生存率的影响。结果：ALDH1蛋白阳性表达率,在膀胱癌与正常膀胱组织中分别为33.94%（37/109）和5.00%（1/20）,差异有统计学意义（P〈0.01）;在非肌层浸润性与肌层浸润性膀胱癌中分别为19.05%（8/42）和43.28%（29/67）,差异有统计学意义（P〈0.01）;在低级别与高级别膀胱癌中分别为13.04%（3/23）和39.53%（34/86）,差异有统计学意义（P〈0.05）;在淋巴转移组与淋巴未转移组膀胱癌组织中分别为50.00%（3/6）和12.90%（4/31）,差异有统计学意义（P〈0.05）;在转移淋巴结及未转移淋巴结组织中分别为50.00%（3/6）和0.00%（0/20）,差异有统计学意义（P〈0.01）。术后随访4-65个月,经Kaplan-Merier分析,ALDH1蛋白阳性表达组患者总生存率为64.9%,阴性表达组为84.7%,差异有统计学意义（P〈0.05）;ALDH1蛋白阳性表达组患者总体无瘤生存率为51.40%,阴性表达组为75.00%,差异有统计学意义（P〈0.05）。结论：肿瘤干细胞标记蛋白ALDH1高表达与浸润性膀胱癌分期和分级及预后有关联,是浸润性膀胱癌预后不良的重要因素。

MRPS5对膀胱癌细胞增殖能力及干性特征的影响

目的探讨线粒体核糖体蛋白S5(mitochondrial ribosomal protein S5,MRPS5)对人膀胱癌细胞的增殖能力及其中干细胞干性特征的影响。方法 Western blot检测人膀胱癌及癌旁正常组织MRPS5的表达;构建靶向干扰MRPS5的慢病毒载体,感染膀胱癌细胞株T24,以干扰Scramble序列作为对照,Western blot检测MRPS5干扰效率;细胞活力实验检测细胞增殖能力;流式细胞术检测细胞周期;细胞成球实验观察成球能力;Western blot检测肿瘤干性转录因子Nanog,Oct4,c-Myc和Sox2的表达;小鼠皮下移植瘤实验观察T24体内成瘤能力。结果 MRPS5在膀胱癌组织中的表达高于癌旁正常组织;慢病毒干扰载体PLKO.1-sh MRPS5有效,且干扰MRPS5表达后T24细胞增殖能力下降(P<0.05),周期阻滞于S期,干性因子表达均下调,成球率无变化(P>0.05)但成球直径明显减小;同时小鼠体内成瘤体积减小[(0.784±0.278)vs(0.500±0.245)cm3,P<0.05],瘤质量减轻[(0.862±0.372)vs(0.412±0.248)g,P<0.05]。结论 MRPS5在膀胱癌中较高表达,且干扰MRPS5表达能抑制T24增殖并抑制T24中的干细胞生物学特征。

CXCR2在膀胱癌干细胞增殖、凋亡及侵袭转移中的作用及机制

目的探讨趋化因子受体2(CXCR2)在膀胱癌干细胞增殖、凋亡及侵袭转移中的作用及机制。方法取膀胱癌肿瘤组织,培养成悬浮肿瘤细胞球,用流式细胞仪筛选出CD44+膀胱癌干细胞。采用Western blotting法检测干细胞标志基因Oct4、Sox2蛋白表达,并检测CXCR2蛋白表达。培养膀胱癌干细胞,将其分为sh-CXCR2组和转染对照组,sh-CXCR2组加入慢病毒转染试剂polybrene与CXCR2敲减慢病毒,转染对照组加入慢病毒转染试剂polybrene与对照scramble。转染72 h后,采用MTS法检测两组细胞增殖率,软琼脂克隆实验观察细胞克隆形成能力,流式细胞仪检测细胞凋亡率,Transwell小室转移实验和Boyden侵袭实验观察细胞转移和侵袭能力,Western blotting法检测两组细胞中凋亡相关蛋白FOXO1A、Bcl-2以及侵袭转移相关蛋白MMP-2、MMP-9的相对表达量。结果流式细胞仪分选出CD44+细胞占全部细胞的2.37%,CD44+细胞中Oct4、Sox2、CXCR2蛋白表达水平高于CD44-细胞(P均<0.05)。与转染对照组比较,sh-CXCR2组细胞增殖率降低,克隆球形成数量减少,细胞凋亡率升高,侵袭和转移实验的穿膜细胞数量减少,细胞中FOXO1A、Bcl-2、MMP-2、MMP-9蛋白表达降低(P均<0.05)。结论CXCR2在膀胱癌干细胞中高表达,抑制其表达可以降低膀胱癌干细胞的增殖、侵袭、转移能力,促进细胞凋亡;其机制可能是通过作用于凋亡相关蛋白FOXO1A、Bcl-2和侵袭转移相关蛋白MMP-2、MMP-9实现的。

膀胱癌T24中肿瘤干细胞样细胞的分离与鉴定

目的观察使用无血清培养基悬浮培养能否从膀胱癌T24中分离出微球体,并证实其是否有肿瘤干细胞的特点。方法使用无血清培养基DMEM/F12添加生长因子EGF、bFGF、胰岛素、B27对膀胱癌T24进行悬浮培养,并从长期增殖能力、克隆形成能力、自我更新能力、对放化疗的抵抗能力、迁移和侵袭能力等方面证实这些微球体是否有肿瘤干细胞的特点。结果从培养的第4天开始长出微球体,微球体细胞比普通贴壁T24细胞有更强的增殖能力和克隆形成能力,对放化疗的抵抗能力更强,有更强的迁移和侵袭能力,微球体有自我更新能力,具有肿瘤干细胞的特点。结论使用无血清悬浮培养可以从T24中分离出微球体,而且这些微球体细胞有肿瘤干细胞的特点。

干细胞标记物OCT4在膀胱癌中的表达及其临床意义

目的探讨干细胞关键转录因子OCT4在膀胱癌患者组织中的表达与临床病理因素及预后的相关性。方法选取河北大学附属医院病理科收集的73例经泌尿外科手术切除的膀胱癌组织(膀胱癌组)及30例癌旁组织(癌旁组)作为标本进行免疫组化染色观察,对比两种OCT4蛋白的表达程度,并分析其与患者的临床病理特征及远期预后的关系。结果膀胱癌组织中OCT4蛋白的阳性表达率(71.23%)显著高于癌旁组织(10.00%)(P<0.05);膀胱癌组织中OCT4蛋白的阳性表达与膀胱癌分化程度、发生血管淋巴结转移、浸润深度有关(P<0.05),与年龄、性别、病理分期无关(P>0.05);膀胱癌组织中OCT4蛋白的阳性表达3年生存率显著低于阴性表达(P<0.05),3年生存中位时间显著短于阴性表达(P<0.05)。结论 OCT4表达与膀胱癌转移有关,对远期预后具有不良影响。

干扰长链非编码RNA CCAT2对膀胱癌细胞J82线粒体功能和肿瘤干细胞样特性的影响

目的探讨干扰长链非编码RNA CCAT2(lncRNA CCAT2)对膀胱癌细胞J82线粒体功能、肿瘤干细胞样特性的影响。方法通过构建lncRNA CCAT2短发卡RNA(shRNA)干扰CCAT2表达,RT-PCR验证并选择其中CCAT2表达量最低的J82细胞系用于后续实验。克隆形成检测细胞增殖、流式细胞仪检测线粒体膜电位变化情况,Western blot检测细胞凋亡相关蛋白水平,显微下观察肿瘤细胞成球情况,流式细胞仪检测各组细胞CD133的表达,Western blot检测OCT4、SOX2、CD44水平。结果三种CCAT2-shRNA J82细胞系中的CCAT2表达量均低于shRNA-NC(P<0.05);CCAT2-shRNA组克隆形成率、c-Myc水平、肿瘤成球直径及成球率、CD133阳性细胞数、OCT4、SOX2、CD44水平低于shRNA-NC组(P<0.05),绿色荧光强度、Bax/Bcl-2、Caspase-3、Caspase-9水平均高于shRNA-NC组(P<0.05)。结论下调lncRNA CCAT2表达量可以抑制J82细胞生长,可能与影响细胞线粒体功能以及肿瘤干细胞样特性有关。

MAGE-A3在人类膀胱癌干细胞中的表达

目的:研究肿瘤相关抗原,黑色素瘤抗原家族A成员3(melanoma antigen family A,3;MAGE-A3),在人类膀胱癌干细胞中的表达情况,并探讨其意义。方法:采用反转录聚合酶链反应(RT-PCR)技术和Western blot技术检测MAGE-A3在人类膀胱癌细胞系T24细胞中及从其中分离出来的具有干细胞特性的T24侧群细胞中的表达情况;采用免疫荧光双标记技术检测MAGE-A3和膀胱癌干细胞的一个标志物CD133在T24侧群细胞中的共表达情况。结果:在mRNA和蛋白水平,MAGE-A3在具有癌干细胞特性的T24侧群细胞中的表达水平明显高于对应的母系T24细胞;MAGE-A3和膀胱癌干细胞标志物CD133在T24侧群细胞中有阳性共表达。结论:MAGE-A3在人类膀胱癌干细胞中有特异性的高表达,有望成为膀胱癌干细胞一个新的、特异性的标志物,及针对膀胱癌干细胞进行免疫治疗的一个新的靶点。

敲减免疫调节蛋白B7-H3基因对膀胱癌细胞恶性增殖、侵袭和干细胞样特性的影响

目的·探讨干扰免疫调节蛋白B7-H3基因对膀胱癌J82细胞的恶性增殖和干细胞样特性的影响。方法·shRNA干扰效率的检测采用反转录聚合酶链式反应(reverse transcription-polymerase chain reaction,RT-PCR)。J82细胞增殖采用克隆形成实验检测。细胞凋亡采用流式细胞术检测。细胞侵袭采用Transwell检测。肿瘤克隆能力采用肿瘤成球实验观察。细胞凋亡、侵袭和干细胞样相关蛋白表达采用蛋白质印迹法(Western blotting)检测。结果·B7-H3在膀胱癌组织及膀胱癌细胞系中高表达(P=0.000)。确定shRNA2为设计的3组shRNAs中干扰B7-H3基因效率最高(P=0.000)。B7-H3干扰抑制了J82细胞的增殖、侵袭、肿瘤克隆能力及干细胞样特性(P=0.000)。并且,B7-H3干扰促进了J82细胞的凋亡(P=0.000)。结论·免疫调节蛋白B7-H3基因干扰可对膀胱癌J82细胞的恶性增殖、侵袭及干细胞样特性产生抑制作用。