N-myc downstream regulated gene 1 inhibition of tumor progression in Caco2 cells

BACKGROUND Invasion and migration are the irreversible stages of colorectal cancer(CRC).The key is to find a sensitive,reliable molecular marker that can predict the migration of CRC at an early stage.N-myc downstream regulated gene 1(NDRG1)is a multifunctional gene that has been tentatively reported to have a strong relationship with tumor invasion and migration,however the current molecular role of NDRG1 in CRC remains unknown.AIM To explore the role of NDRG1 in the development of CRC.METHODS NDRG1 stably over-expressed Caco2 cell line was established by lentiviral infection and NDRG1 knock-out Caco2 cell line was established by CRISPR/Cas9.Furthermore,the mRNA and protein levels of NDRG1 in Caco2 cells after NDRG1 over-expression and knockout were detected by real-time polymerase chain reaction and western blot.The cell proliferation rate was measured by the cell counting kit-8 method;cell cycle and apoptosis were detected by flow cytometry;invasion and migration ability were detected by the 24-transwell method.RESULTS NDRG1 over-expression inhibited Caco2 proliferation and the cell cycle could be arrested at the G1/S phase when NDRG1 was over-expressed,while the number of cells in the G2 phase was significantly increased when NDRG1 was knocked out.This suggests that NDRG1 inhibited the proliferation of Caco2 cells by arresting the cell cycle in the G1/S phase.Our data also demonstrated that NDRG1 promotes early cell apoptosis.Invasion and migration of cells were extensively inhibited when NDRG1 was over-expressed.CONCLUSION NDRG1 inhibits tumor progression in Caco2 cells which may represent a potential novel therapeutic strategy for the treatment of CRC.

Regulation of HIF-1 α to Expression of N-myc Downstream Regulated Gene 1 in Colorectal Carcinoma

Plasmid expressing small interfering RNA （siRNA） against HIF-1α （pSilence-2.1-U6-siRNA） was constructed and transfected into LS174T cells in hypoxia condition.After expression of siRNA against HIF-1 α in LS174T cells, expressions of HIF-1 α and N-myc downstream regulated gene 1 （NDRG1） gene were inhibited significantly. HIF-1 cta transcripts were positive in 67.7% （42/62） and 44.4% （8/18） of colorectal adenocarcinoma and adenoma, re- spectively. The mean percentage of cells with positive hybridization of HIF-1 α mRNA increases with the development from Duke stage A to stage C＋D （p〈 0.05）. The positive staining rate of NDRG1 protein was significant higher in than that in colorectal adenoma colorectal adenocarcinoma group group （p〈 0.05）. The level of HIF-1 a transcripts was positively correlated with the level of NDRG1 protein （p 〈 0.05） during colorectal tumor progression. HIF-1α and its down stream gene NDRG1 may play roles in tumor progression of human colorectal carcinoma.

Inhibition of N-Myc down regulated gene 1 in in vitro cultured human glioblastoma cells

AIM: To study short ds RNA oligonucleotides(si RNA)as a potent tool for artificially modulating gene expression of N-Myc down regulated gene 1(NDRG1) gene induced under different physiological conditions(Normoxia and hypoxia) modulating NDRG1 transcription, m RNA stability and translation. METHODS: A cell line established from a patient with glioblastoma multiforme. Plasmid DNA for transfections was prepared with the Endofree Plasmid Maxi kit. From plates containing 5 × 107 cells, nuclear extracts were prepared according to previous protocols. The p SUPERNDRG1 vectors were designed, two sequences were selected from the human NDRG1 c DNA(5'-GCATTATTGGCATGGGAAC-3' and 5'-ATGCAGAGTAACGTGGAAG-3'. reverse transcription polymerase chain reaction was performed using primers designed using published information on β-actin and hypoxia-inducible factor(HIF)-1α m RNA sequences in Gen Bank. NDRG1 m RNA and protein level expression results under different conditions of hypoxia or reoxygenation were compared to aerobic control conditions using the Mann-Whitney U test. Reoxygenation values were also compared to the NDRG1 levels after 24 h of hypoxia(P < 0.05 was considered significant).RESULTS: si RNA- and iodoacetate(IAA)-mediated downregulation of NDRG1 m RNA and protein expression in vitro in human glioblastoma cell lines showed a nearly complete inhibition of NDRG1 expression when compared to the results obtained due to the inhibitory role of glycolysis inhibitor IAA. Hypoxia responsive elements bound by nuclear HIF-1 in human glioblastoma cells in vitro under different oxygenation conditions and the clearly enhanced binding of nuclear extracts from glioblastoma cell samples exposed to extreme hypoxic conditions confirmed the HIF-1 Western blotting results. CONCLUSION: NDRG1 represents an additional diagnostic marker for brain tumor detection, due to the role of hypoxia in regulating this gene, and it canrepresent a potential target for tumor treatment in human glioblastoma. The si RNA method can represent an elegant alternative to modulate the expression of the hypoxia induced NDRG1 gene and can help to monitor the development of the cancer disease treatment outcome through monitoring the expression of this gene in the patients undergoing the different therapeutic treatment alternatives available nowadays.

N-MYC及NDRG1在胃癌组织中的表达及对胃癌细胞生物学特性的影响

目的分析N-MYC及N-MYC下游调节基因1(NDRG1)在胃癌组织中的表达及对胃癌细胞生物学特性的影响。方法收集2021年1月至2023年5月于该院行手术切除且经病理确诊为胃癌的82例患者的胃癌组织及癌旁正常组织,采用实时荧光定量PCR(qPCR)检测N-MYC、NDRG1 mRNA相对表达量,收集患者临床资料,分析N-MYC、NDRG1 mRNA表达与患者临床病理特征关系。选择对数生长期NCI-N87细胞,将N-MYC干扰质粒(si-N-MYC)与其阴性对照(si-NC)分别转染到NCI-N87细胞中,记为si-NC组、si-N-MYC组;将si-N-MYC分别与anti-NC、anti-NDRG1共转染至NCI-N87细胞中,记为si-N-MYC+anti-NC组、si-N-MYC+anti-NDRG1组。采用CCK-8实验检测细胞增殖活性,Transwell侵袭实验检测细胞侵袭能力,Western blotting法检测细胞中N-MYC、NDRG1蛋白表达。结果胃癌组织N-MYC mRNA相对表达量高于癌旁组织(P<0.05),NDRG1 mRNA相对表达量低于癌旁组织(P<0.05)。不同胃癌TNM分期、淋巴结转移、远处转移患者N-MYC、NDRG1 mRNA表达差异有统计学意义(P<0.05)。与si-NC组比较,si-N-MYC组细胞增殖和侵袭能力下降(P<0.05),NDRG1蛋白表达下调(P<0.05)。与si-N-MYC+anti-NC组比较,si-N-MYC+anti-NDRG1组细胞增殖、侵袭能力增加(P<0.05)。N-MYC可靶向调控NDRG1,敲低NDRG1可逆转N-MYC对细胞产生的生物学作用。结论胃癌组织N-MYC mRNA表达上调、NDRG1 mRNA表达下调,二者参与胃癌的发生发展过程,并对胃癌细胞增殖、侵袭等恶性生物学行为有重要调控作用。

增殖细胞核抗原和细胞分化相关基因N-myc下游调节基因1在乳腺癌中的表达及意义

目的探讨增殖细胞核抗原(PCNA)、细胞分化相关基因N-myc下游调节基因1(NDRG1)在乳腺癌中的表达。方法选择乳腺手术切除标本90例进行切片,应用免疫组织化学链霉亲和素-生物素复合物(SABC)法检测45例乳腺癌组织、23例乳腺增生组织、22例癌旁正常乳腺组织中PCNA和NDRG1蛋白的表达情况,并分析其与乳腺癌生物学行为的关系。结果 PCNA在癌旁正常乳腺组织、乳腺增生组织和乳腺癌组织中的表达率分别为36.3%、62.5%和88.9%,PCNA在癌旁正常乳腺组织中的表达明显低于乳腺增生组织(P<0.05)和乳腺癌组织(P<0.05)。NDRG1在癌旁正常乳腺组织、乳腺增生组织和乳腺癌组织中的表达率分别为63.6%、30.4%和15.5%,NDRG1在癌旁正常乳腺组织中的表达明显高于乳腺增生组织(P<0.05)和乳腺癌组织(P<0.05)。PCNA与NDRG1表达呈负相关(r=-0.679,P<0.05)。结论 PCNA与NDRG1共同参与乳腺癌的发生与发展,联合检测PCNA和NDRG1蛋白有助于判断乳腺癌的恶性程度。

三叶因子2和N-myc下游调节基因1在不同子宫内膜组织中的表达

目的 探讨三叶因子2（TFF2）和N-myc下游调节基因1（NDRG1）在不同子宫内膜组织中的表达,为早期诊断子宫内膜癌提供新的生物学指标。方法 收集珠海市人民医院经手术切除并经病理检查确诊为子宫内膜癌组织157例,另选择同期经手术切除并经病理检查确诊的子宫内膜不典型增生组织30例及其他病因手术切除的正常子宫内膜20例,分别检测其TFF2和NDRG1蛋白的表达情况,并分析TFF2和NDRG1蛋白的表达与子宫内膜癌临床病理因素的关系。结果 与正常子宫内膜和子宫内膜不典型增生组织比较,TFF2在子宫内膜癌组织中的阳性表达率显著降低（P〈0.05）,但NDRG1在子宫内膜癌组织中的阳性表达率显著升高（P〈0.01）。TFF2在Ⅰ、Ⅱ期子宫内膜癌组织中的阳性表达率显著高于Ⅲ~Ⅳ期（P〈0.05）;高、中分化子宫内膜癌组织中TFF2的阳性表达率显著高于低分化组织及其他类型（P〈0.01）。与深肌层浸润的子宫内膜癌比较,浅肌层浸润的子宫内膜癌组织中TFF2的阳性表达率显著升高（P〈0.05）;与有淋巴结转移的子宫内膜癌比较,无淋巴结转移的子宫内膜癌组织中TFF2的阳性表达率显著升高（P〈0.01）。而高、中度分化的子宫内膜癌组织中NDRG1的阳性表达率显著低于低分化及其他类型（P〈0.05）。浅肌层浸润的子宫内膜癌组织中NDRG1的阳性表达率显著低于深肌层浸润（P〈0.01）,与无淋巴结转移的子宫内膜癌比较,有淋巴结转移的子宫内膜癌组织中NDRG1的阳性表达率显著升高（P〈0.01）。结论 在子宫内膜组织中,TFF2表达的缺失及NDRG1蛋白的高表达可能与子宫内膜癌的发生发展有重要关系,有望在子宫内膜癌的早期诊断、判断是否存在侵袭转移等临床评估中发挥作用。

上调N-myc下游调节基因1表达对胰腺癌细胞增殖及凋亡的作用

目的观察磷酸化增强型绿色荧光蛋白-N-myc下游调节基因N3(p EGFP-NDRG1-N3)上调Nmyc下游调节基因1(NDRG1)表达的胰腺癌细胞增殖、细胞周期及凋亡的影响并探讨其机制。方法以Western blot法对PANC-1、BXPC-3、CAPAN-2、SW1990细胞中NDRG1表达进行检测;构建过表达质粒p EGFPNDRG1-N3转染CAPAN-2细胞,以免疫荧光、Western blot法及实时定量逆转录-聚合酶链反应(RT-PCR)检测上调效率;采用甲基噻唑基四唑(MTT)法检测转染后细胞增殖;碘化丙啶(PI)法检测细胞周期;流式细胞术检测细胞凋亡。结果 Western blot显示,NDRG1在4组细胞株中均有表达,而在低分化细胞(PANC-1)中的表达量要高于中分化(BXPC-3)及高分化细胞株(CAPAN-2、SW1990)(P<0.05);免疫荧光显示,p EGFP-NDRG1-N3组荧光细胞数占总细胞数>70%,NDRG1在蛋白及m RNA水平表达上调;在m RNA水平,NDRG1表达上调后Parp、Cleaved Parp、p-P53、Cleaved-Capase3无改变(t=1.456、1.164、2.914和1.075,P>0.05)。在蛋白水平,Parp表达下调,Cleaved Parp表达上调,p-P53下调,Cleaved-Capase3下调(t=6.104、12.273、3.691和14.227,P<0.05);MTT显示,在96和120 h与p EGFP-N3组比较,p EGFP-NDRG1-N3转染后CAPAN-2细胞增殖能力增强(t=8.176和2.246,P<0.05);PI法显示,转染p EGFP-NDRG1-N3的CAPAN-2细胞停留在G1期比例增高,G2及S期比例减少,与p EGFP-N3组比较,差异有统计学意义(t=3.651、4.133和3.092,P<0.05);p EGFPNDRG1-N3凋亡低于p EGFP-N3组,差异有统计学意义(t=9.161,P<0.01)。结论胰腺癌细胞NDRG1表达上调促进胰腺癌细胞增殖,抑制凋亡,促进细胞进入G1期,可作为胰腺癌治疗新的靶向候选基因。

结直肠癌组织中lncRNA CCAT2和NDRG1的表达及意义

目的探讨结直肠癌(CRC)患者组织中长链非编码RNA(lncRNA)结肠癌相关转录物2(CCAT2)、N-myc下游调节基因(NDRG)1的表达及与临床病理特征及预后的关系。方法选取2018年2月至2020年2月在南通市中医院行CRC根治性手术治疗的96例CRC患者作为研究对象。采用实时荧光定量PCR检测组织中lncRNA CCAT2、NDRG1 mRNA表达,采用免疫组织化学检测组织中NDRG1蛋白表达,采用Kaplan-Meier曲线分析不同lncRNA CCAT2、NDRG1 mRNA表达组患者的预后差异,采用多因素Cox回归分析CRC预后影响因素。结果与癌旁组织比较,癌组织中lncRNA CCAT2表达较高,NDRG1 mRNA表达及蛋白阳性率较低,差异有统计学意义(P<0.05)。与TNM分期Ⅰ~Ⅱ期、无淋巴结转移比较,TNM分期Ⅲ期、有淋巴结转移的CRC患者癌组织中lncRNA CCAT2表达较高,NDRG1 mRNA表达较低(P<0.05)。lncRNA CCAT2高表达组3年累积生存率低于lncRNA CCAT2低表达组,而NDRG1 mRNA高表达组3年累积生存率高于NDRG1 mRNA低表达组,差异有统计学意义(P<0.05)。TNM分期、淋巴结转移,lncRNA CCAT2、NDRG1 mRNA是CRC预后影响因素(P<0.05)。结论CRC组织中lncRNA CCAT2表达升高,NDRG1表达降低,二者均参与CRC肿瘤的进展,可作为评估CRC患者生存预后的新指标。

增殖细胞核抗原、人类N-myc下游调节基因1在肝细胞性肝癌中的表达及临床意义

目的：研究增殖细胞核抗原（PCNA）及人类N-myc下游调节基因1（NDRG1）在人肝细胞性肝癌中的表达情况,探讨其与肝癌生物学行为的关系及临床意义。方法：选择有存档的原发性肝癌标本58例,肝硬化34例,正常肝组织标本15例,用H-E染色观察组织形态,用免疫组织化学SABC检测PCNA和NDRG1的表达。结果：肝癌组织中PCNA表达明显高于肝硬化组织和正常组织;在肝硬化组织和正常肝组织中,PCNA的表达没有差异;肝癌中PCNA的表达与患者的性别、年龄、HbsAg阳性、AFP水平、部位和肿瘤的直径无关。NDRG1在正常肝组织、肝硬化组织、肝癌组织中表达逐渐减弱;肝硬化组与正常肝组织组相比,差异无统计学意义,在肝癌组织中NDRG1与患者的性别、年龄、HbsAg阳性、AFP水平、部位和肿瘤的直径无关。PCNA及NDRG1在肝癌组织中的表达呈负相关。结论：PCNA、 NDRG1在肝癌发生、发展过程中起着重要的作用,联合检测可以为肿瘤的早发现、早诊断、早治疗提供判断依据。

N-myc下游调控基因1在呼吸系统疾病中的研究进展

N-myc下游调控基因1(N-myc downstream regulated gene-1,NDRG1)是NDRG家族的第一个成员,与低氧和应激相关。NDRG1广泛分布在全身多种组织器官中,具有特有的分子结构和化学修饰。在肺中NDRG1主要表达在呼吸道组织内,其表达水平和化学修饰与多种呼吸系统疾病的发生发展有密切关系,包括感染性疾病、慢性气道炎性疾病、低氧相关疾病(如肺损伤、急性呼吸窘迫综合征)等,同时在肿瘤低氧微环境、肿瘤进展及耐药等方面也发挥重要作用。本文就NDRG1在呼吸系统疾病中的相关研究进展作一综述。

Lipoxin A4 Ameliorates Lipopolysaccharide-lnduced A549 Cell Injury through Upregulation of N-myc Downstream-Regulated Gene-1

Background： Lipoxin A4 （LXA4） can alleviate lipopolysaccharide （LPS）-induced acute lung injury （ALl） and acute respiratory distress syndrome through promoting epithelial sodium channel （ENaC） expression in lung epithelial cells. However, how LXA4 promote ENaC expression is still largely elusive. The present study aimed to explore genes and signaling pathway involved in regulating ENaC expression induced by LXA4. Methods： A549 cells were incubated with LPS and LXA4, or in combination, and analyzed by quantitative real-time polymerase chain reaction （qRT-PCR） of ENaC-α/γ. Candidate genes affected by LXA4 were explored by transcriptome sequencing ofA549 cells. The critical candidate gene was validated by qRT-PCR and Western blot analysis ofA549 cells treated with LPS and LXA4 at different concentrations and time intervals. LXA4 receptor （ALX） inhibitor BOC-2 was used to test induction of candidate gene by LXA4. Candidate gene siRNA was adopted to analyze its influence on A549 viability and ENaC-α expression. Phosphoinositide 3-kinase （PI3K） inhibitor LY294002 was utilized to probe whether the PI3K signaling pathway was involved in LXA4 induction of candidate gene expression. Results： The A549 cell models of ALl were constrticted and subjected to transcriptome sequencing. Among candidate genes, N-myc downstream- regulated gent- 1 （NDRG 1 ） was validated by real-time-PCR and Western blot. NDRG 1 mRNA was elevated in a dose-dependent manner of LXA4, whereas BOC-2 antagonized NDRG 1 expression induced by LXA4. NDRG I siRNA suppressed viability of LPS-treated A549 cells （treatment vs. control, 0.605± 0.063 vs. 0.878 ± 0.083, P = 0.040） and ENaC-α expression （treatment vs. control, 0.458 ± 0.038 vs. 0.711 ± 0.035, P = 0.008）. LY294002 inhibited NDRG 1 （treatment vs. control, 0.459 ± 0.023 vs. 0.726 ± 0.020, P 0.001 ） and ENaC-α （treatment vs. control, 0.236 ± 0.021 vs. 0.814 ±0.025, P 〈 0.001 ） expressions and serum- and glucocorticoid-inducible kinase I phosphorylation （treatment vs. control, 0.442± 0.024 vs. 1.046 ± 0.082, P = 0.002）, indicating the PI3K signaling pathway was involved in regulating NDRG 1 expression induced by LXA4. Conclusion： Our research uncovered a critical role of NDRG1 in LXA4 alleviation of LPS-induced A549 cell injury through mediating PI3K signaling to restore ENaC expression.

自噬蛋白Beclin-1与N-myc下游调控基因2在食管鳞状细胞癌中的表达及其临床意义

目的探索自噬蛋白Beclin-1和N-myc下游调控基因2(NDRG2)在食管鳞状细胞癌(ESCC)中的表达,并探讨两种蛋白作为ESCC预后分子标志物的临床价值。方法采用免疫组织化学染色检测Beclin-1与NDRG2在121例ESCC组织中的表达,通过Pearson相关分析两者表达与临床病理参数的关系。根据Beclin-1与NDRG2的表达情况将所有患者分为2组,高、低表达组的生存概率通过Kaplan-Meier曲线计算,Log-rank检验用于生存分析的比较。采用Cox比例风险模型进行单因素和多因素分析,确定ESCC患者的独立预后因子。结果免疫组织化学染色分析显示Beclin-1蛋白在121例ESCC及癌旁组织中的阳性表达率分别为40.5%(49/121)和59.5%(68/121),差异有统计学意义(χ^(2)=5.973,P=0.015)。NDRG2蛋白在ESCC组织中的阳性表达率亦明显低于癌旁组织,差异有统计学意义(46.3%vs.61.2%;χ^(2)=5.385,P=0.020)。Beclin-1低表达者有更为频繁的淋巴结转移(χ^(2)=6.158,P=0.013)和更晚的TNM分期(χ^(2)=4.538,P=0.033),而NDRG2低表达与更晚的T分期(χ^(2)=6.607,P=0.010)和TNM分期(χ^(2)=5.744,P=0.017)相关。Kaplan-Meier曲线显示,Beclin-1低表达与高表达患者的3年总体生存(OS)率分别为44.3%和60.9%,差异有统计学意义(χ^(2)=5.696,P=0.017)。NDRG2低表达者的预后亦明显低于NDRG2高表达者,3年OS率分别为43.9%和59.2%(χ^(2)=9.004,P=0.003)。单、多因素Cox比例风险模型分析表明,Beclin-1低表达(HR=1.727,95%CI:1.017~2.934,P=0.043)、NDRG2低表达(HR=1.671,95%CI:1.023~2.730,P=0.040)与TNMⅡ~Ⅲ期(HR=3.823,95%CI:2.133~6.852,P<0.001)是ESCC患者预后不良的独立预测因素。结论Beclin-1和NDRG2表达在ESCC中明显下调,且与患者不良预后相关,其可能是预测ESCC患者生存的预后标志物。

卵巢子宫内膜异位囊肿患者血清APRIL与NDRG1的水平表达及其临床价值研究

目的观察血清增殖诱导配体(a proliferation inducing ligand,APRIL),N-myc下游调节基因1(N-myc downstream regulated gene 1,NDRG1)水平变化,并分析其对卵巢子宫内膜异位囊肿(ovarian endometriomas,OEM)的诊断价值。方法选取2021年7月~2022年7月在自贡市第一人民医院就诊的132例OEM患者作为观察组,并进行定期随访,根据患者预后病情有无复发分为复发组(n=50)和未复发组(n=82)。同期在该院体检的健康者78例为对照组。采用酶联免疫吸附法(enzyme linked immunosorbent assay,ELISA)检测血清中APRIL和NDRG1水平;并对复发组和未复发组的一般资料进行比较;采用Logistic回归分析影响OEM预后的相关因素;用Pearson法分析OEM患者血清APRIL与NDRG1表达相关性;绘制受试者工作特征(receiver operating characteristic,ROC)曲线分析血清APRIL和NDRG1对OEM的诊断价值。结果与对照组相比,APRIL水平(35.28±6.81ng/ml vs 26.37±3.19ng/ml)和NDRG1水平(124.39±15.67μg/L vs 9.67±10.82μg/L)升高,差异具有统计学意义(t=10.864,17.278,均P<0.05)。与未复发组比较,复发组血清APRIL(40.38±7.88ng/ml vs 32.16±6.18ng/ml)和NDRG1(132.04±19.83μg/L vs 119.73±13.16μg/L)水平升高,差异具有统计学意义(t=6.668,4.287,均P<0.05)。Logistic回归分析显示,血清APRIL和NDRG1水平是影响OEM患者预后的危险因素(Waldχ^(2)=11.839,28.437,均P<0.001)。Pearson法分析结果显示,OEM患者血清APRIL水平与NDRG1水平呈正相关(r=0.439,P<0.001)。血清APRIL,NDRG1水平联合诊断OEM的曲线下面积(AUC)为0.849,灵敏度和特异度分别为73.95%,85.37%,优于APRIL和NDRG1单独预测(Z=2.644,2.094,P=0.008,0.036)。结论子宫内膜异位囊肿患者血清APRIL和NDRG1水平升高,二者联合对子宫内膜异位囊肿诊断具有较高的临床价值,且与子宫内膜异位囊肿患者的预后密切相关。

Correlation of LSD1 and NDRG1 gene expression in ovarian cancer tissue with cancer cell migration and invasion

Objective: To study the correlation of LSD1 and NDRG1 gene expression in ovarian cancer tissue with cancer cell migration and invasion. Methods: Patients with ovarian cancer who underwent surgical resection in Fufeng County People's Hospital between March 2014 and July 2017 were selected as the research subjects, and the ovarian cancer tissue and adjacent tissue were collected after surgical resection to determine the expression of LSD1, NDRG1, migration genes and invasion genes. Results: LSD1, YKL40, COX2, Twist, IFITM1, CatL, CTHRC1, MMP2 and FUNDC1 mRNA expression in ovarian cancer tissue were significantly higher than those in adjacent tissue whereas NDRG1, E-cadherin and Wnt5a mRNA expression were significantly lower than those in adjacent tissue;YKL40, COX2, Twist, IFITM1, CatL, CTHRC1, MMP2 and FUNDC1 mRNA expression in ovarian cancer tissue with high LSD1 expression were significantly higher than those in ovarian tissue with low LSD1 expression whereas E-cadherin and Wnt5a gene mRNA expression were significantly lower than those in ovarian tissue with low LSD1 expression. Conclusion: The high LSD1 expression and low NDRG1 expression in ovarian cancer tissue can promote the migration and invasion of cancer cells.

NDRG1通过ERK通路增强肝细胞癌对索拉菲尼的耐药

目的 探究N-myc下游调控基因1(NDRG1)对肝细胞癌(HCC)的作用,以及NDRG1是否影响HCC对索拉菲尼(Sorafenib)的敏感性。方法 通过TCGA数据库预测NDRG1在HCC中的表达水平,并通过蛋白质印迹(WB)实验和免疫组织化学(IHC)染色进行验证。构建NDRG1敲除细胞系进行体外实验,通过肿瘤功能学实验细胞计数试剂盒8(CCK-8)、EdU染色、细胞划痕、Transwell实验研究NDRG1及联合Sorafenib对HCC细胞增殖、迁移与侵袭以及凋亡的影响。利用裸鼠皮下荷瘤进行体内实验,研究NDRG1和Sorafenib对HCC成瘤的影响;通过WB实验和IHC染色确定NDRG1调节HCC对Sorafenib敏感性的通路。结果 WB实验和IHC染色显示,NDRG1在HCC中高表达,与TCGA数据结果一致。肿瘤功能学实验结果表明NDRG1敲除或Sorafenib刺激使HCC细胞增殖、迁移及侵袭能力减弱,肿瘤细胞凋亡增加,而NDRG1敲除联合Sorafenib使HCC细胞增殖、迁移与侵袭能力进一步减弱,肿瘤细胞凋亡进一步增加(P<0.000 1)。小鼠皮下荷瘤模型结果表明NDRG1敲除或Sorafenib刺激使荷瘤体积及质量减小,而NDRG1敲除联合Sorafenib使荷瘤体积及质量进一步减小(P<0.000 1)。WB和IHC结果表明NDRG1敲除联合Sorafenib可降低Erk1/2的磷酸化水平。结论 NDRG1在HCC中高表达,高表达NDRG1促进HCC细胞增殖、迁移和侵袭能力,并抑制肿瘤细胞凋亡。NDRG1通过ERK信号通路增强HCC对Sorafenib的耐药。

食管鳞癌组织中NDRG1 mRNA和蛋白的表达

目的:探讨食管鳞癌组织中NDRG1mRNA和蛋白的表达情况及其与临床病理因素的关系。方法:分别采用RT PCR和免疫组织化学SP法检测49例食管鳞癌组织(分化程度Ⅰ级14例,Ⅱ级23例,Ⅲ级12例;有淋巴结转移21例,无淋巴结转移28例)、23例癌旁不典型增生黏膜组织及49例正常食管黏膜组织中NDRG1mRNA和蛋白的表达。结果:食管鳞癌组织中NDRG1mRNA相对含量低于癌旁不典型增生黏膜组织及正常食管黏膜组织(P<0.05或0.01);不同分化程度的食管鳞癌组织之间NDRG1mRNA相对含量差异无统计学意义(P>0.05);伴淋巴结转移的食管鳞癌组织与无淋巴结转移的食管鳞癌组织NDRG1mRNA相对含量差异无统计学意义(P>0.05)。癌旁不典型增生组织及食管鳞癌组织中NDRG1蛋白()阳性率(3/23和4/49)均低于正常黏膜组织的43/49(P<0.01);食管鳞癌组织中NDRG1蛋白表达与癌组织的分级及有、无淋巴结转移无关(P均>0.05)。结论:食管鳞癌组织中NDRG1mRNA和蛋白表达降低,其低表达可能与食管鳞癌发生有关。

1,25-(OH)_2VitD_3对食管癌细胞分化相关基因NDRG1表达的影响

目的了解1,25-(OH)2VitD3对食管癌细胞分化相关基因NDRG1表达的影响。方法采用1,25-(OH)2VitD3作用于人食管癌EC9706细胞,应用免疫组化和RT-PCR方法分别检测1,25-(OH)2VitD3作用不同时间后NDRG1基因的表达。结果1,25-(OH)2-VitD3作用24h～5dNDRG1基因蛋白和mRNA均显著高于对照组水平(P<0.05)。结论1,25-(OH)2VitD3可上调EC9706细胞分化相关基因NDRG1表达,促使其分化。

NDRG1、P21及VEGF在肺腺癌组织中的表达及临床意义

目的:观察N-myc下游调节基因1(N-myc downstream regulated gene1,NDRG1)、P21及血管内皮生长因子(vascular endothelial growth factor,VEGF)基因在肺腺癌中的表达及在肺腺癌发生、发展中的作用及意义。方法:应用免疫组织化学法检测20例正常肺组织和94例肺腺癌组织中NDRG1、P21及VEGF蛋白的表达情况,并分析三者表达与临床病理参数及患者预后的相关性。结果:在正常肺组织及肺腺癌组织中,NDRG1阳性率分别为90.0%(18/20)和52.1%(49/94),P21阳性率分别为80.0%(16/20)和33.0%(31/94),VEGF阳性率分别为20.0%(4/20)和53.2%(50/94),3种蛋白阳性率比较差异均具有统计学意义(P均<0.05)。肺腺癌组织中NDRG1、P21及VEGF的表达与肺腺癌患者年龄、性别、组织分化程度及TNM分期均无相关性(P均>0.05),而与淋巴结转移明显相关(P<0.05)。Kaplan-Meier生存分析显示,NDRG1、P21和VEGF表达与生存明显相关(P均<0.01)。结论:肺腺癌组织中NDRG1和P21表达下调,而VEGF表达上调,联合检测三者的表达可能对判断预后具有重要价值。

维生素D_3对EC9706细胞增殖、裸鼠移植瘤生长及NDRG1蛋白表达的影响

目的:观察1,25-(OH)2维生素D3对食管癌EC9706细胞细胞增殖、细胞周期、食管癌细胞裸鼠移植瘤生长及对NDRG1蛋白表达的影响。方法:采用0.3μmol/L的1,25-(OH)2维生素D3作用于EC9706细胞后,MTT法检测肿瘤细胞的增殖情况,流式细胞仪检测细胞周期的变化。BALB/c小鼠荷瘤后,用5μg/kg1,25-(OH)2维生素D3溶液皮下注射于移植瘤周围,观察移植瘤生长情况,并采用免疫组织化学方法检测裸鼠移植瘤组织中NDRG1蛋白表达水平。实验中均以未经1,25-(OH)2维生素D3处理作为对照组。结果:①MTT实验结果显示,1,25-(OH)2维生素D3作用1～5d时各组吸光度均低于对照组,差异有统计学意义(P<0.05);随着1,25-(OH)2维生素D3作用时间的延长,细胞增殖抑制率逐渐升高(1d:7.4%,3d:21.1%,5d:23.8%)。②细胞周期检测结果显示,不同培养时间组G1期细胞分别与对照组比较,差异均有统计学意义(P<0.05)。③与对照组相比,1,25-(OH)2维生素D3可上调NDRG1蛋白表达水平。结论:1,25-(OH)2维生素D3可抑制食管癌细胞增殖,并通过上调NDRG1的表达而抑制食管癌裸鼠移植瘤的生长。

宫颈鳞状细胞癌组织中NDRG-1、COX-2、VEGF的表达及其临床意义

目的:观察N-myc下游调节基因-1(N-myc downstream regulated gene-1,NDRG-1)、环氧合酶-2(cyclooxygenase-2,COX-2)及血管内皮生长因子(vascular endothelial growth factor,VEGF)在宫颈鳞状细胞癌组织中的表达,分析其在宫颈鳞状细胞癌发生发展中的作用及意义。方法:采用免疫组织化学法检测80例宫颈鳞状细胞癌患者癌组织和15例正常宫颈组织中NDRG-1、COX-2及VEGF蛋白表达情况;分析宫颈鳞状细胞癌组织中3种蛋白表达的相关性,并分析其表达与临床病理因素及患者预后的关系。结果:与正常宫颈组织比较,宫颈鳞状细胞癌组织中NDRG-1阳性表达率明显降低(P<0.01);COX-2与VEGF阳性表达率明显升高(P<0.01)。NDRG-1、COX-2及VEGF蛋白的阳性表达与宫颈鳞状细胞癌患者的年龄及肿瘤大小无关(P>0.05),而与肿瘤组织病理学分级、FIGO分期及淋巴结转移密切相关(P<0.01)。Kaplan-Meier生存分析显示,宫颈鳞状细胞癌组织中NDRG-1表达阳性者生存期较长,COX-2及VEGF表达阳性者生存期较短。结论:宫颈鳞状细胞癌组织中NDRG-1表达降低,而COX-2及VEGF表达增加,三者表达的联合检测可能对判断宫颈鳞状细胞癌的预后具有重要价值。