Hugl-1 induces apoptosis in esophageal carcinoma cells both in vitro and in vivo

AIM: To determine whether the human giant larvae homolog 1 gene (Hugl-1/Llg1/Lgl1) exerts tumor suppressor effects in esophageal cancer. METHODS: We constructed a Hugl-1 expression plasmid, pEZ-M29-Hugl1, for gene transfection. We transfected the pEZ-M29-Hugl1 plasmid into Eca109 esophageal cancer cell lines with Lipofectamine 2000 to overexpress Hugl-1. Real-time reverse transcription-polymerase chain reaction (RT-PCR) and Western blotting were performed to determine the effects of the plasmid on Hugl-1 expression. In vitro cell proliferation and apoptosis were examined separately by cell counting Kit-8 (CCK-8) assay, flow cytometry, and Western blotting before and after the transfection of the plasmid into Eca109 cells. Cell cycle distribution was assessed with flow cytometry. The effect of Hugl-1 overexpressing on tumor growth in vivo was performed with a xenograft tumor model in nude mice. Expression of Hugl-1 in xenograft tumor was analyzed by immunohistochemistry.The transferase-mediated dUTP nick end-labeling (TUNEL) technique was performed to detect and quantitate apoptotic cell. RESULTS: The transfection efficiency was confirmed with real-time RT-PCR and Western blotting. Our results show that compared with control groups the mRNA levels and protein levels of Hugl-1 in pEZ-M29-Hugl1-treated group were remarkably increased (P < 0.05). The CCK-8 assay demonstrated that the growth of cells overexpressing Hugl-1 was significantly lower than control cells. Cell cycle distribution showed there was a G 0 /G 1 cell cycle arrest in cells overexpressing Hugl-1 (64.09% ± 3.14% vs 50.32% ± 4.60%, 64.09% ± 3.14% vs 49.13% ± 2.24%). Annexin V-fluorescein isothiocyanate revealed that apoptosis was significantly increased in cells overexpressing Hugl-1 compared with control group (17.33% ± 4.76% vs 6.90% ± 1.61%, 17.33% ± 4.76% vs 6.27% ± 0.38%). Moreover, we found that Hugl-1 changes the level of the anti-apoptotic protein Bcl-2 and the proapoptotic protein Bax and the activation of both caspase-3 and caspase-9. With a TUNEL assay, we found that Hugl-1 markedly increased the apoptosis rate of Eca109 cells in vivo (60.50% ± 9.11% vs 25.00% ± 12.25%). It was shown that Hugl-1 represents a significantly more effective tumor suppressor gene alone in a xenograft tumor mouse model. This data suggest that Hugl-1 inhibited tumor growth and induced cell apoptosis in vivo . CONCLUSION: These results suggest that Hugl-1 induces growth suppression and apoptosis in a human esophageal squamous cell carcinoma cell line both in vitro and in vivo .

Transcription factor EGR-1 inhibits growth of hepatocellular carcinoma and esophageal carcinoma cell lines

AIM: The transcription factor EGR-1 (early growth response gene-1) plays an important role in cell growth, differentiation and development. It has identified that EGR-1 has significant transformation suppression activity in some neoplasms, such as fibrosarcoma, breast carcinoma. This experiment was designed to investigate the role of egr-1 in the cancerous process of hepatocellular carcinoma (HCC) and esophageal carcinoma (EC), and then to appraise the effects of EGR-1 on the growth of these tumor cells. METHODS: Firstly, the transcription and expression of egr-1 in HCC and EC, paracancerous tissues and their normal counterpart parts were detected by in situ hybridization and immunohistochemistry, with normal human breast and mouse brain tissues as positive controls. Egr-1 gene was then transfected into HCC (HHCC, SMMC7721) and EC (ECa109) cell lines in which no egr-1 transcription and expression were present. The cell growth speed, FCM cell cycle, plate clone formation and tumorigenicity in nude mice were observed and the controls were the cell lines transfected with vector only. RESULTS: Little or no egr-1 transcription and expression were detected in HCC, EC and normal liver tissues. The expression of egr-1 were found higher in hepatocellular paracancerous tissue (transcription level P=0.000; expression level P=0.143, probably because fewer in number of cases) and dysplastic tissue of esophageal cancer (transcription level P=0.000; expression level P=0.001). The growth rate of egr-1-transfected HHCC (HCC cell line) cells and ECa109 (EC cell line) cells was much slower than that of the controls. The proportion of S phase cell, clone formation and tumorigenicity were significantly lower than these of the controls' (decreased 45.5% in HHCC cells and 34.1% in ECa109 cells; 46.6% and 41.8%; 80.4% and 72.6% respectively). There were no obvious differences between SMMC7721 (HCC) egr-1-transfected cells and the controls with regard to the above items. CONCLUSION: The decreased expression of egr-1 might play a role in the dysregulation of normal growth in the cancerous process of HCC and EC. Egr-1 gene of transfected HHCC and ECa109 cells showed obvious suppression of the cell growth and malignant phenotypes, but no suppression in SMMC7721 (HCC cell line) cells.

GSTM1,GSTT1,GSTP1 and CYP1A1 genetic polymorphisms and susceptibility to esophageal cancer in a French population:Different pattern of squamous cell carcinoma and adenocarcinoma

AIM:To evaluate the association between CYP1A1 and GSTs genetic polymorphisms and susceptibility to esophageal squamous cell carcinoma(SCC)and esophageal adenocarcinoma(ADC)in a high risk area of northwest of France. METHODS:A case-control study was conducted to investigate the genetic polymorphisms of these enzymes (CYPIAI*2C and GSTP1 exon 7 Val alleles,GSTMI*2/*2 and GSTTl *2/*2 null genotypes).A total of 79 esophageal cancer cases and 130 controls were recruited. RESULTS:GSTMI*2/*2 and CYPIAI*IA/*2C genotype frequencies were higher among squamous cell carcinomas at a level dose to statistical significance(OR =1.83,95% CI 0.88-3.83,P=0.11;OR=3.03,95% CI 0.93-9.90,P=0.07, respectively).For GSTP1 polymorphism,no difference was found between controls and cases,whatever their histological status.Lower frequency of GSTT1 deletion was observed in ADC group compared to controls with a statistically significant difference(OR=13.31,95% CI 1.66-106.92,P<0.01). CONCLUSION:In SCC,our results are consistent with the strong association of this kind of tumour with tobacco exposure.In ADC,our results suggest 3 distinct hypotheses: (1)activation of exogenous procarcinogens,such as small halogenated compounds by GSTT1;(2)contribution of GSTT1 to the inflammatory response of esophageal mucosa,which is known to be a strong risk factor for ADC, possibly through leukotriene synthesis;(3)higher sensitivity to the inflammatory process associated with intracellular depletion of glutathione.

Experimental and clinic-opathologic study on the relationship between transcription factor Egr-1 and esophageal carcinoma

AIM: To observe the growth suppression effect of exogenous introduction of early growth response gene-1 (Egr-1 gene) on esophageal carcinoma tissue as well as on esophageal carcinoma cell line Eca109 and to explore the potential application of Egr-1 gene in gene therapy of tumor. METHODS: Eukaryotic expression vector of PCMV-Egr-1 plasmid was introduced into Eca109 cell line which expressed no Egr-1 protein originally with lipofectamine transfection method. The introduction and expression of PCMV-Egr-1 plasmid into Eca109 cell line was confirmed by G418 selection culture, PCR amplification of neogene contained in the vector, Western blot analysis and immunocytochemical analysis. The cell growth curve, soft agar colony formation rate and tumorigenicity in SCID mice were examined to demonstrate the growth suppression effect of exogenous Egr-1 gene on Eca109 cell line. The Egr-1 mRNA and Egr-1 protein were also detected in 50 surgical specimens of esophageal carcinoma by in situ hybridization and immunohistochemistry. RESULTS: Exogenous Egr-1 gene was introduced successfully into Eca109 cell line and expressed Egr-1 protein stably. The transfected Eca109 cell line grew more slowly than control Eca109 as shown by cell growth curves, the soft agar colony formation rate (4.0% vs 6.9%, P 【 0.01) and the average growth rate of tumor in SCID mice (35.5 +/- 7.6 vs 65.8 +/- 7.6, P 【 0.05). The expression level of Egr-1 mRNA and protein significantly increased in dysplastic epithelia adjacent to cancer rather than in cancer tissues (65.8% vs 20.0% by ISH and 57.9% vs 0.01). CONCLUSION: Exogenous Egr-1 gene shows the strong effect of growth inhibition in Eca109 cell line. Egr-1 in the cancer tissue shows down-regulated expression that supports the inhibited function of Egr-1 in cancer growth and suggests Egr-1 may have an important role in gene therapy of esophageal carcinoma.

Relationships of early esophageal cancer with human papillomavirus and alcohol metabolism

BACKGROUND It is well known that an alcohol consumption habit together with inactive heterozygous aldehyde dehydrogenase-2(ALDH2)is an important risk factor for the development of esophageal squamous cell carcinoma(ESCC).It remains controversial whether human papillomavirus(HPV)infection contributes to the occurrence/development of ESCC.There has been no study in which the relationship between ESCC and HPV in addition to alcohol dehydrogenase-1B(ADH1B)and ALDH2 genotypes was evaluated.AIM To evaluate relationships between HPV infection and development of esophageal cancer,particularly early esophageal cancer,based on ADH1B/ALDH2 polymorphisms.METHODS We conducted an exploratory retrospective study using new specimens,and we enrolled 145 patients who underwent endoscopic resection for superficial ESCC and had been observed for more than two years by both physical examination and endoscopic examination in Hokkaido University Hospital.Saliva was collected to analyze genetic polymorphisms of ADH1B/ALDH2.We performed in situ hybridization for resected specimens to detect HPV by using an HPV type 16/18 probe.RESULTS HPV was detected in 15(10.3%)of the 145 patients with ESCC.HPV-positive rates in inactive ALDH2*1/*2 and ALDH2*1/*1+*2/*2 were 10.8%and 9.8%,respectively(P=1.00).HPV-positive rates in slow-metabolizing ADH1B*1/*1 and ADH1B*1/*2+*2/*2 were 12.0%and 10.0%,respectively(P=0.72).HPV-positive rates in the heavy or moderate alcohol consumption group and the light or rare consumption group were 11.1%and 8.7%,respectively(P=0.68).HPV-positive rates in the heavy smoking group and the light or no smoking group were 11.8%and 8.3%,respectively(P=0.59).The 3-year incidence rates of secondary ESCC or head and neck cancer after initial treatment in the HPV-positive and HPVnegative groups were 14.4%and 21.4%(P=0.22),respectively.CONCLUSION In the present situation,HPV status is considered to be less important than other risk factors,such as alcohol consumption,smoking habit,ADH1B/ALDH2 polymorphisms,and HPV status would therefore have no effect on ESCC risk management.

GENISTEIN INHIBITS PROLIFERATION OF HUMAN ENDOMETRIAL ENDOTHELIAL CELL IN VITRO

Objective To explore the effect of genistein on proliferation of human endometrial endothelial cells （HEECs） and glandular epithelium. Methods In vitro HEECs and human endometrial cancer-1B cell （HEC-1B ） were cultured with 0, 1, 10, 50, 100, and 200 μmol/L of genistein alone or indicated concentrations of genistein combined with 0.2 or 1 nmol/L 17β- estradiol （ 17β-E2）. Cell proliferation was determined by [ 3H ] -thymidine incorporation and cell cycle was measured by flow cytometry. Results After 96 hours of treatment, genistein inhibited the proliferation of HEECs in a dose-dependent manner. The stimulation index reduced from 100% （ without genistein treatment ） to about 1% （ 200 μmol/L genistein ）. HEECs were arrested at G1/0 and G2/M phase when treated with genistein for 96 hours. When the concentration of genistein was 200 μmol/L, the percentages of HEECs at G1/0, G2/M, and S phase were 96. 0%, 2.1%, and 1.9%, respectively. However, when HEECs were treated without genistein, the percentages of HEECs at G1/0, G2/M, and S phase were 76. 7%, 8.5%, and 14. 7%, respectively. 1713-E2 could not influence the effects of genistein on the proliferation of HEECs. Meanwhile, genistein could suppress the proliferation of HEC-1B. If the stimulation index of HEC-IB was defined as 100% when HEC-1B was treated with different doses of 1713-E2 （without genistein）, it was 67%, 19%, as well as 32% when cell was supplemented with 200 μmol/L genistein combined with 0, 0. 2, or 1 nmol/L 17β-E2, respectively. Conclusion Genistein at the concentration of 200 μmol/L can sufficiently inhibit the proliferation of HEECs and endometrial glandular epithelium simultaneously in vitro.

血清SCC-Ag、VEGF、UHRF1水平联合预测食管鳞癌根治术后复发的价值

目的探讨血清人鳞状细胞癌相关抗原(SCC-Ag)、血管内皮生长因子(VEGF)、环指域1(UHRF1)水平联合预测食管鳞癌根治术后复发的价值。方法回顾性分析2017年5月至2019年6月因食管鳞癌于郑州大学第一附属医院接受根治术治疗的116例患者的临床资料。术前均检测血清SCC-Ag、VEGF、UHRF1水平,比较不同临床病理特征患者各血清指标。术后均随访3 a,根据是否复发将患者分为复发组(56例)和未复发组(60例),并比较两组血清SCC-Ag、VEGF、UHRF1水平和临床病理特征。采用Cox回归模型分析食管鳞癌根治术后复发的危险因素,并绘制受试者工作特征(ROC)曲线分析血清SCC-Ag、VEGF、UHRF1水平联合对食管鳞癌根治术后复发的预测价值。结果最大肿瘤直径>5 cm、有淋巴结转移、TNM分期Ⅲ期、低分化程度患者血清SCC-Ag、VEGF、UHRF1水平均高于最大肿瘤直径≤5 cm、无淋巴结转移、TNM分期Ⅰ~Ⅱ期、高/中分化程度患者(P<0.05);复发组血清SCC-Ag、VEGF、UHRF1水平和最大肿瘤直径>5 cm、有淋巴结转移、TNM分期Ⅲ期、低分化程度占比均高于未复发组(P<0.05);Cox回归模型分析结果显示,在未校正因素时,血清SCC-Ag、VEGF、UHRF1水平均是食管鳞癌患者根治术后3 a内复发的危险因素(RR=2.978、3.031、3.126,P<0.05),校正性别、年龄、肿瘤部位、最大肿瘤直径、淋巴结转移、TNM分期、分化程度后仍是术后3 a内复发的危险因素(RR=1.939、2.112、2.235,P<0.05);ROC曲线分析结果显示,血清SCC-Ag、VEGF、UHRF1水平联合预测食管鳞癌根治术后复发的灵敏度和曲线下面积(AUC)分别为94.64%、0.919,均高于各指标单独预测(P<0.05),其特异度与各指标单独预测比较差异无统计学意义(P>0.05)。结论血清SCC-Ag、VEGF、UHRF1水平与食管鳞癌患者临床病理特征和术后复发均具有一定的相关性,对术后复发均具有预测价值,但三者联合预测价值更高。

三氧化二砷对人食管癌细胞株EC-1的放射增敏作用

目的探讨三氧化二砷(As2O3)对食管癌离体肿瘤细胞EC-1的放射增敏作用,并探讨其机制。方法利用多靶单击数学模型拟合放射剂量-细胞存活曲线,观察As2O3对食管癌细胞株EC-1的放射增敏作用。流式细胞法观察As2O3对细胞周期分布及细胞凋亡的影响。结果 As2O3对食管癌细胞株EC-1有明显的放射增敏效应,3μmol/L As2O3作用48 h的放射增敏比为1.285。药物作用后G2/M期细胞比例增加,G0/G1期和S期细胞比例减少;细胞凋亡指数增加,与对照组相比,差异有统计学意义(P<0.05)。结论 As2O3对食管癌细胞株EC-1有明显的放射增敏效应。放射增敏的机制可能与As2O3抑制EC-1细胞的修复能力、使细胞周期阻滞在G2/M期、G0/G1期和S期细胞减少以及凋亡增加有关。

食管鳞癌组织中hPOT1、hTERT及p53的表达

目的探讨食管鳞癌组织中端粒保护蛋白1(hPOT1)、端粒酶催化亚基(hTERT)及p53的表达及其意义。方法采用免疫组织化学技术检测82例食管鳞癌组织中hPOT1、hTERT及p53的表达情况。结果82例鳞癌组织中,hPOT1蛋白阳性表达率为78·05%(64/82),hTERT蛋白阳性表达率为68·29%(56/82),p53蛋白的阳性表达率为65·85%(54/82),它们与淋巴结转移、病理分期密切相关(P<0·05)。结论联合检测hPOT1、hTERT及p53蛋白的表达对判断食管鳞癌的预后有一定的指导意义。

脱氧雪腐镰刀菌烯醇对人食管上皮细胞TAP-1和LMP-2表达的影响

目的：探讨不同浓度脱氧雪腐镰刀菌烯醇（DON）处理,体外原代培养的人正常食管上皮细胞TAP-1、LMP-2表达的变化。方法：采用Western blot和RT-PCR技术从蛋白水平和mRNA水平上分析不同浓度的DON处理24小时,体外培养的人正常食管上皮细胞TAP-1、LMP-2分子表达的变化规律及其量-效关系。结果：不同浓度（50、100、1 000、2 000μg/L）DON处理人食管上皮细胞24小时后,DON各处理组食管上皮细胞TAP-1蛋白的Western blot半定量检测结果分别为0.47±0.22、0.28±0.16、0.24±0.18和0.21±0.19,统计分析表明DON 100、1 000、2 000μg/L处理组与对照组相比差异有统计学意义（P〈0.05）。相关分析表明,在0~2000μg/L浓度范围内,随DON处理浓度增高,食管上皮细胞TAP-1蛋白的表达量逐渐降低（r=-0.595,n=4,P〈0.01）。RT-PCR结果发现,经不同浓度DON处理食管上皮细胞TAP-1mRNA的相对表达量虽然呈现先升高后降低的趋势,但与对照组相比无统计学差异。DON各处理组LMP-2蛋白的Western blot半定量检测结果分别为2.25±1.03、3.31±1.35、1.90±1.19和2.12±0.22均高于空白对照组（0.91±0.21）,其中100μg/L处理组相对表达量最高,差异有统计学意义（P〈0.05）。RT-PCR结果,DON 100μg/L处理组的LMP-2 mRNA的相对表达量最高为2.23±0.56,明显高于对照组,差异有统计学意义（P〈0.05）。其余处理组差异无统计学意义。结论：DON可剂量依赖地抑制体外培养的人正常食管上皮细胞的TAP-1蛋白的表达,但对TAP-1的mRNA未见显著影响。DON（100μg/L）可以促进食管上皮细胞LMP-2蛋白和mRNA表达,其余各浓度未见明显影响。

沉默单核细胞趋化蛋白-1基因降低人食管癌EC109细胞的迁移及侵袭能力

单核细胞趋化蛋白-1(monocyte chemoattractant protein-1,MCP-1)是白色脂肪细胞分泌的炎症趋化刺激因子,属于趋化因子CC亚族,可促进肿瘤血管形成和细胞外基质降解,从而促进肿瘤细胞的浸润与转移。沉默MCP-1基因可显著抑制恶性肿瘤生长及转移,但其作用的分子机制尚不完全清楚。本研究应用小干扰RNA技术沉默人食管癌EC109细胞中MCP-1表达。细胞划痕试验显示,与对照组相比,沉默MCP-1基因可明显抑制食管癌EC109细胞迁移能力。Transwell侵袭实验显示,沉默MCP-1基因后,EC109细胞侵袭能力降低。Western印迹试验和RT-PCR试验揭示,沉默MCP-1基因后,细胞中MMP-7、MMP-9、TGF-β_1及VEGF表达水平显著下降。研究结果提示,沉默MCP-1基因可通过抑制MMP-7、MMP-9、TGF-β_1及VEGF表达,降低癌细胞迁移及侵袭能力。

hMLH1和RASSF1A在食管癌组织中的表达及其与患者预后的关系

目的:探讨食管鳞癌组织中hMLH1和RASSF1A基因表达及其对预后的影响.方法:采用原位杂交技术检测hMLH1基因、免疫组织化学法检测RASSF1A基因在60例食管鳞癌患者中的表达,应用Cox回归模型和Kaplan-Meier生存曲线分析其与患者预后的关系.结果:在食管鳞癌组织中hMLH1 mRNA表达显著低于正常黏膜组织(41.67%vs90.00%,P<0.01),RASSF1A蛋白表达低于食管正常黏膜组织(80%vs100%,P<0.05).hMLH1和RASSF1A的表达与TNM分期、食管癌浸润深度、淋巴结转移和肿瘤大小相关(均P<0.05),但与民族无关;RASSF1A与hMLH1表达呈正相关(r=0.338,P<0.01);本组病例5年总生存率为35%(21/60),单因素生存分析表明,食管癌hMLH1高表达组5年生存率高于低表达组,差异有统计学意义(P<0.05);RASSF1A高表达组较低表达组有生存优势,但差异无统计学意义;Cox模型多因素分析表明,hMLH1和RASSF1A不是影响生存期的独立因素,而肿瘤浸润深度和TNM分期均是影响生存期的独立因素(P<0.05).结论:hMLH1和RASSF1A在食管癌组织中表达均较低,其表达水平与食管肿瘤的发生发展有一定的关系,结合临床病理可作为判断预后的指标.

D-氨基葡萄糖衍生物对Eca-109细胞内活性氧、线粒体膜电位的影响

目的:探讨2-(3-羧基-1-丙酰氨基)-2-脱氧-D-葡萄糖(2-[(3-carboxy-1-oxoprogy1)amino]-2-deoxy-D-Glucose,COPADG)诱导Eca-109细胞凋亡的机制。方法:不同浓度COPADG作用于人食管癌Eca-109细胞24h,检测Eca-109细胞的抑制率、凋亡率、细胞内活性氧(ROS)、线粒体跨膜电位。结果:Eca-109细胞凋亡率与COPADG浓度呈正相关(rs=1.0,P<0.01);Eca-109细胞线粒体膜电位水平与Eca-109细胞凋亡率相关(rs=1.0,P<0.01);ROS水平与Eca-109细胞凋亡率呈正相关(rs=1.0,P<0.01);ROS水平与Eca-109细胞线粒体膜电位水平呈负相关(rs=1.0,P<0.01)。结论:COPADG可促进Eca-109细胞凋亡,提高Eca-109细胞内ROS水平,并降低线粒体膜电位水平。实验结果提示COPADG提高ROS水平,降低Eca-109细胞线粒体膜电位水平,启动细胞凋亡通路,促使Eca-109细胞凋亡,并且线粒体膜电位的下降是通过提高ROS实现的。

EGFR、Her-2、HIF-1α、p53对进展期食管鳞癌新辅助化疗疗效的预测价值

目的:探讨食管鳞癌相关因子EGFR、Her-2、HIF-1α和p53对进展期食管鳞癌新辅助化疗疗效的预测价值。方法:回顾性分析日照市人民医院2011年1月-2015年1月行紫杉醇联合顺铂方案新辅助化疗的进展期食管鳞癌(Ⅲ期)患者94例,采用免疫组化方法检测食管鳞癌组织中EGFR、Her-2、HIF-1α和p53的表达情况,应用RECIST1.1标准和病理组织学相结合方法行化疗疗效评估,Logistic多因素回归分析各指标与化疗疗效关系。结果:本研究组患者新辅助化疗总有效率为56.38%(53/94),全部为部分缓解。疾病稳定占41.49%(39/94),疾病进展占2.13%(2/94)。新辅助化疗前后各因子表达差异无统计学意义(均P>0.05)。Her-2表达阳性、阴性者化疗有效率分别为81.82%(9/11)、53.01%(44/83),两者比较差异有统计学意义(P=0.01)。p53表达阳性、阴性者化疗有效率分别为31.37%(16/51)、86.05%(37/43),两者差异有统计学意义(P<0.01)。Her-2阳性表达同时p53阴性表达者7例,其中化疗有效5例。EGFR和HIF-1α表达与化疗敏感性无关(P>0.05)。多因素分析显示,Her-2和p53是新辅助化疗的独立影响因素(均P<0.05)。结论:Her-2和p53作为新辅助化疗独立影响因子,可在化疗前对疗效进行预测,可能对患者新辅助化疗选择提供临床依据。

食管鳞癌患者血清IGF-1的检测分析

目的:探讨食管鳞癌患者血清IGF-1的浓度及其临床意义。方法:设立食管鳞癌组合正常对照组。以化学发光法检测65例食管鳞癌患者和30例正常人血清IGF-1的浓度。结果:正常健康人血清IGF-1的含量是(195.35±48.21)ng/ml,食管鳞癌患者为(1 082.29±301.24)ng/ml,明显高于正常对照组(P<0.01),且血清IGF-1水平随临床病理分期的进展而逐步增高(P<0.05)。结论:血清IGF-1有可能作为食管鳞癌诊断或病情监测的一个指标。

hRFT1基因单核苷酸多态性与新疆哈萨克族食管鳞癌的相关性研究

目的:检测新疆哈萨克族食管鳞癌中hRFT1基因rs346821多态性位点基因型及等位基因型的分布。探讨hRFT1基因多态性与新疆哈萨克族食管鳞癌的相关性。方法:(1)运用基质辅助激光解析电离时间飞行质谱仪(MALDI-TOF-MS)对206例哈萨克族食管鳞癌及217例哈萨克族正常对照的hRFT1基因多态性分布进行检测;(2)采用SPSS13.0统计软件进行统计学处理,计算对照组基因型频率以确定符合Hardy-Weinberg平衡,组间基因型及等位基因型分布频率比较采用χ2检验。结果:(1)hRFT1基因rs346821位点A/G多态中G/G、A/G、A/A基因型频率在病例组别为18.6%、70.1%、11.3%,在对照组分别为45.5%、46.5%、8%,经检验差异有统计学意义(χ2=30.713,P=0.00);(2)hRFT1基因rs346821位点A/G多态中G、A等位基因频率在病例组分别为53.7%、46.3%,在对照组分别为68.8%、31.2%,经检验差异有统计学意义(χ2=18.061,P=0.00)。结论:hRFT1基因rs346821位点基因型及等位基因型与新疆哈萨克族食管鳞状细胞癌具有相关性。

真核起始因子4E反义寡核苷酸对人食管癌EC-1细胞中真核起始因子4E表达的影响

目的:探讨真核起始因子4E(eIF4E)反义寡核酸(ASODN)对人食管癌EC-1细胞中eIF4E表达的影响。方法:将针对eIF4E不同基因位点的2条反义寡核苷酸(ASODN1、2)和1条无义寡核苷酸(N-ODN)转染EC-1细胞(设5、10、15μmol/L3个转染浓度),分别培养24、48、72h,并设空脂质体转染作为空白对照,采用免疫细胞化学和原位杂交方法检测转染后细胞中eIF4E蛋白和mRNA表达的变化。结果:ASODN1、2转染EC-1细胞培养24、48、72h后,各组中eIF4E蛋白和mRNA的表达均降低,2者分别与空白对照组相比,差异均有统计学意义(P<0.05);ASODN1、2组每个时间段内随浓度增加ASODN抑制效应增强,差异具有统计学意义(F=9.423、10.284、10.496、7.621、8.420和9.089,P<0.05),组间相同时间点、相同浓度的抑制效应比较差异无统计学意义(P>0.05);NODN组和空白对照组对eIF4E的表达均无抑制效应。结论:特异性的ASODN能有效抑制人食管癌EC-1细胞中eIF4E的表达。

三氧化二砷对食管癌细胞株EC-1的生长抑制作用

目的:探讨三氧化二砷((Arsenic trioxide,As2O3)对食管癌细胞株EC-1生长抑制作用及机制。方法:采用MTT法检测不同浓度As2O3(0.5、1、2、4、8、16、32、64μmol/L)在不同时间段(24、48、72 h)对EC-1细胞增殖的抑制率,计算半数抑制率(IC50)值。流式细胞术检测细胞凋亡及细胞周期变化。结果:三氧化二砷对食管癌EC-1细胞具有增殖抑制作用,呈剂量-效应和时间-效应关系(P<0.05)。IC50约为18.74μmol/L。As2O3可使细胞阻滞在G2/M期,使G0/G1期、S期细胞比例减少,增加细胞凋亡,差异具有统计学意义(P<0.05)。结论:As2O3能抑制食管癌EC-l细胞株的增殖,具有明显的量效和时效关系。其机制可能与改变周期,增加其细胞凋亡有关。

hMLH1蛋白在食管鳞状细胞癌和不典型增生组织中的表达

目的:探讨同一食管癌患者食管的鳞状细胞癌组织、不典型增生组织、正常鳞状上皮组织中错配修复基因1(hu-man mutl homolog1,hMLH1)的蛋白表达情况,深入研究它与食管鳞状细胞癌发生发展的关系。方法:取92例食管鳞状细胞癌患者的病变组织,其病理切片中鳞状细胞癌组织、不典型增生组织和正常鳞状上皮组织均存在,采用免疫组织化学的方法,检测hMLH1蛋白在3种不同组织中的表达,并分析其与性别、年龄、分化程度、浸润深度、肿瘤分期、淋巴结转移等临床病理参数之间的关系。结果:hMLH1蛋白在食管鳞状细胞癌组织、不典型增生组织、正常鳞状上皮组织细胞核中的阳性表达率分别为36.96%、56.52%、84.78%,鳞状细胞癌组织和不典型增生组织均显著低于正常食管鳞状上皮组织(P<0.01)。鳞状细胞癌组织中hMLH1蛋白表达阴性者,年龄较阳性者大(P<0.05);hMLH1蛋白表达与肿瘤分期、淋巴结转移等有明显相关性(P<0.05)。结论:hMLH1基因缺失可能在早期就参与了食管鳞状细胞癌的发生过程,hMLH1蛋白可能抑制或延缓食管鳞状细胞癌的发生和发展。

血清HO-1、SCC-Ag在中晚期食管鳞癌术后化疗中的变化及临床意义

目的:探讨血清血红素加氧酶-1(HO-1)、人鳞状细胞癌相关抗原(SCC-Ag)在中晚期食管鳞癌术后化疗中的变化及临床意义。方法:选2015年9月至2017年9月行体检的174例健康人群及同期收治的116例中晚期食管鳞癌患者,分别抽取血清进行HO-1、SCC-Ag水平的监测并比较;分别于化疗前后进行上述指标的测定,并分析其HO-1、SCC-Ag水平与临床分期及病理分级之间的关系。结果:食管癌患者HO-1阳性表达率(93.97%)、SCC-Ag水平(2.49±0.63)μg/L均高于健康体检者[5.75%、(0.51±0.11)μg/L],差异有统计学意义(P<0.05)。中、晚期食管鳞癌患者术后化疗后HO-1阳性表达率(72.55%、80.00%)、SCC-Ag水平[(1.98±0.56)μg/L、(3.76±0.97)μg/L]明显低于化疗前HO-1阳性表达率(90.20%、96.92%)和SCC-Ag水平[(2.34±0.78)μg/L、(4.08±0.98)μg/L],差异有统计学意义(P<0.05)。晚期食管鳞癌患者HO-1阳性表达率、SCC-Ag水平高于中期食管鳞癌,差异有统计学意义(P<0.05);肿瘤分化程度越低,HO-1阳性表达率、SCC-Ag水平越高,中、低分化食管鳞癌患者HO-1阳性表达率、SCC-Ag水平明显高于高分化食管鳞癌患者,差异有统计学意义(P<0.05)。结论:中晚期食管鳞癌患者血清HO-1、SCC-Ag水平明显高于正常人,血清HO-1、SCC-Ag在中晚期食管鳞癌术后化疗后降低,血清HO-1、SCC-Ag水平与临床分期呈正相关,血清HO-1、SCC-Ag水平可以作为中晚期食管鳞癌患者的诊断和化疗疗效观察的重要指标。