Hypermethylation of tumor suppressor and tumor-related genes in neoplastic and non-neoplastic gastric epithelia

A number of tumor suppressor and tumor-related genes exhibit promoter hypermethylation with resultant gene silencing in human cancers.The frequencies of methylation differ among genes and genomic regions within CpG islands in different tissue types.Hypermethylation initially occurs at the edge of CpG islands and spreads to the transcription start site before ultimately shutting down gene expression.When the degree of methylation was quantitatively evaluated in neoplastic and non-neoplastic gastric epithelia using DNA microarray analysis,highlevel methylation around the transcription start site appeared to be a tumor-specific phenomenon,although multiple tumor suppressor genes became increasingly methylated with patient age in non-neoplastic gastric epithelia.Quantitative analysis of DNA methylation is a promising method for both cancer diagnosis and risk assessment.

Aberrant methylation of secreted protein acidic and rich in cysteine gene and its significance in gastric cancer

BACKGROUND Aberrant methylation in DNA regulatory regions could downregulate tumor suppressor genes without changing the sequences.However,our knowledge of secreted protein acidic and rich in cysteine(SPARC)and its aberrant methylation in gastric cancer(GC)is still inadequate.In the present research,we performed fundamental research to clarify the precise function of methylation on SPARC and its significance in GC.AIM To investigate promoter methylation and the effects of the SPARC gene in GC cells and tissues and to evaluate its clinical significance.METHODS Plasmids that overexpressed the SPARC gene were transfected into human GC BGC-823 cells;non-transfected cells were used as a control group(NC group).Quantitative real-time polymerase chain reaction and western blotting(WB)were then used to detect the expression of SPARC.Methylation-specific polymerase chain reaction was executed to analyze the gene promoter methylation status.Cell viability was measured by the cell counting kit-8 assay.The migration and invasion ability of cells were detected by scratch assays and transwell chamber assays,respectively.Cell cycle events and apoptosis were observed with a flow cytometer.RESULTS The expression of SPARC mRNA in GC tissues and cells was significantly lower and showed differing degrees of hypermethylation,respectively,than that in normal adjacent tissues and control cells.Treatment with 5-Aza-2’-deoxycytidine(5-Aza-Cdr)was able to restore the expression of SPARC and reverse promoter hypermethylation.Overexpression of the SPARC gene significantly inhibited proliferation,migration,and invasion of GC cells,while also causing cell cycle arrest and apoptosis;the NC group exhibited the opposite effects.CONCLUSION This study demonstrated that SPARC could function as a tumor suppressor and might be silenced by promoter hypermethylation.Furthermore,in GC cells,SPARC inhibited migration,invasion,and proliferation,caused cell cycle arrest at the G0/G1 phase,and promoted apoptosis.

Role of RECK methylation in gastric cancer and its clinical significance

AIM:To investigate the relation between RECK methylation and clinicopathological characteristics of gastric cancer patients and evaluate the role of RECK methylation in peritoneal metastasis of gastric cancer.METHODS:Methylation of RECK gene in 40 paired samples of gastric cancer and its corresponding adjacent normal mucosa,lymph nodes and peritoneal irrigation fluid was detected by methylation-specific polymerase chain reaction.RESULTS:Aberrant methylation of RECK gene was detected in 27.5%(11/40)of the adjacent normal mucosa samples,in 47.5%(19/40)of gastric cancer samples,in 57.1%(12/21)of the lymph node samples,and in 35%(14/40)of peritoneal irrigation fluid samples,respectively,with a significant difference between the adjacent normal mucosa and lymph node samples(P=0.023).Presence of RECK methylation in the primary tumor samples was significantly correlated with tumor invasion(P=0.023).The accuracy of RECK methylation in peritoneal lavage fluid samples for the diagnosis of peritoneal metastasis of gastric cancer was 72.5%(26/40),with a sensitivity of 66.7%(6/9) and a specificity of 74.2%(23/31).CONCLUSION:Aberrant methylation of RECK gene may provide useful information for the early diagnosis and treatment of peritoneal metastasis of gastric cancer.

卡瑞利珠单抗联合伊立替康治疗胃癌效果及对血清BARD1、STAT1影响

目的探讨卡瑞利珠单抗联合伊立替康治疗胃癌的效果及对血清乳腺癌1号基因相关环指蛋白(BARD1)和转录活化蛋白1(STAT1)的影响。方法选取2016年4月—2021年11月收治的胃癌120例,按照治疗方法不同将其分为观察组和对照组2组各60例。观察组给予卡瑞利珠单抗联合伊立替康治疗,对照组给予卡瑞利珠单抗治疗。比较2组治疗后临床效果,治疗后1年生存和复发情况,治疗前后血清肿瘤标志物、免疫功能指标、血清BARD1和STAT1,以及治疗期间毒副作用情况。结果治疗后,观察组总有效率(85.0%,51/60)高于对照组(70.0%,42/60)(P<0.05)。治疗后1年,观察组生存期长于对照组,复发率低于对照组(P<0.05,P<0.01)。治疗后,CD4+、CD4+/CD8+和STAT12组高于治疗前,且观察组高于对照组;血清糖类抗原199、癌胚抗原、CD8+、BARD12组低于治疗前,且观察组低于对照组(P<0.05)。治疗期间,2组毒副作用总发生率比较差异无统计学意义(P>0.05)。结论卡瑞利珠单抗联合伊立替康治疗胃癌患者临床效果较好,可降低血清肿瘤标志物水平,改善免疫功能,还可下调BARD1,上调STAT1,且安全性较好。

胃癌血清肿瘤相关基因超甲基化检测及其意义

目的:探讨检测胃癌患者血清中肿瘤相关基因超甲基化的可行性及其意义。肿瘤患者的血清中游离DNA存在质或量的变化,是可能的肿瘤标志物。DNA甲基化不改变DNA序列和遗传密码,具有可逆性,被认为是基因转录调控的表观遗传机制之一。抑癌基因启动子超甲基化通常导致基因的转录失活,其功能的丧失,参与肿瘤的发生。方法:通过甲基化特异性PCR(MSP)检测52例胃癌组织和配对血清的hMLH1、E-cadherin、GSTP1、p15和p16基因的启动子超甲基化。20例健康体检者血清作为对照。结果:在胃癌组织中检测到hMLH1、E-cadherin、GSTP1、p15和p16基因的启动子超甲基化率分别为28.8%、76.9%、23.1%、59.6%和69.2%;在患者血清中检测到hMLH1、E-cadherin、GSTP1、p15和p16基因的启动子超甲基化率分别为13.5%、38.5%、15.4%、25.0%和30.8%。84.7%的患者血清可以检测到异常甲基化。所有血清中检测到异常甲基化的患者,其肿瘤组织也能检测到相应基因的异常甲基化。对照组血清未检测到任何异常甲基化。结论:MSP检测血清异常甲基化是一种具有较高灵敏度和特异性的方法,可以在大部分胃癌患者血清中同时检测到多个肿瘤相关基因的异常甲基化,可以将其作为胃癌诊断的辅助手段。

胃癌患者血清抑癌基因启动子超甲基化测定的临床意义

目的探讨胃癌患者血清中抑癌基因超甲基化检测的临床意义。方法随机收集2011～2013年上海市静安区中心医院进行胃镜检查的患者,32例胃癌患者为胃癌组,29例萎缩性胃炎为萎缩性胃炎组和30例健康者为健康对照组。应用甲基化特异性PCR（MSP）方法,测定血清Ras相关区域家族基因1a（RASSFA1）基因、人类相关转录因子3（Runx3）基因、错配修复蛋白MutL同源物1（hmLH1）基因、多肿瘤抑制基因1（MTS1）也称P16基因、上皮E钙粘蛋白（E-Cadherin）基因、组织因子途径抑制物2（TFPI-2）基因启动子甲基化状态。结果胃癌组血清RASSF1A、RUNX3、hmLH1、P16、E-Cadherin、TFPI-2基因超甲基化阳性率分别为21.9%,40.6%,21.9%,34.4%,28.1%,28.1%;萎缩性胃炎组分别为3.5%,13.8%,0.0%,6.9%,3.5%,6.9%;对照组仅检出RUNX3基因启动子甲基化,阳性率3.5%;胃癌组血清6种基因启动子甲基化阳性率均明显高于萎缩性胃炎组和健康对照组（P〈0.05）。联合血清中6种基因启动子甲基化对胃癌诊断灵敏度为76.7%,较单独一个基因明显升高（P〈0.05）;特异性为86.5%,与RUNX3基因比较,差异无统计学意义（P〉0.05）,与其他5个基因单独测定特异性降低（P〈0.05）。结论 MSP检测能检测到血清中RASSF1A、RUNX3、hmLH1、P16、E-Cadherin、TFPI-2基因启动子超甲基化。6个基因启动子联合测定对胃癌诊断的灵敏度更高,可为胃癌的诊断、治疗以及判断预后提供新方法或依据。

血清TFPI-2基因甲基化在胃癌诊断中的临床价值

目的通过测定组织及血清组织因子途径抑制物2(TFPI-2)基因甲基化,探讨其作为一种肿瘤标志物对胃癌诊断的临床价值。方法收集32例胃癌、29例萎缩性胃炎作为研究对象,以30例不排除浅表性胃炎的正常对象作为对照。应用甲基化特异性聚合酶链反应(MSP)方法,测定组织及血清TFPI-2基因甲基化状态。应用电化学发光免疫法测定癌胚抗原(CEA)、糖类抗原199(CA199)。结果组织TFPI-2基因甲基化检出率胃癌组为53.13%、萎缩性胃炎组为37.93%、对照组为3.33%。胃癌组明显高于对照组(P<0.05)。血清TFPI-2基因甲基化检出率胃癌组为28.13%,萎缩性胃炎组为6.90%,对照组未检出。胃癌组明显高于萎缩性胃炎组(P<0.05)和对照组(P<0.05)。血清TFPI-2基因甲基化检测灵敏度为28.13%,特异性为96.61%。血清检出阳性占组织检出阳性的比率为37.93%。胃癌组血清TFPI-2基因甲基化与性别、年龄、Borrmann's分期、CEA和CA199检测结果无关(P>0.05)。胃癌组血清TFPI-2基因甲基化与CEA、CA199阳性检出率分别为28.13%、21.88%、18.75%。联合3项阳性检出率为53.13%,显著高于3项各自单独检测(P<0.05)。结论血清TFPI-2基因甲基化来源于组织,其对胃癌诊断特异性较高,但灵敏度较差。联合检测血清CEA、CA199有利于提高其灵敏度。血清TFPI-2基因甲基化测定对胃癌的诊断有一定价值。

胃癌诊断的研究进展

胃癌是最常见的恶性肿瘤之一,因早期胃癌缺乏特异性临床表现,难以与胃良性疾病相鉴别,致使早期胃癌漏诊率及误诊率均较高,发现时多已属中晚、期,失去最佳的手术时机,严重影响预后,故早期发现、诊断及治疗是提高胃癌患者生存率,降低病死率的关键。该文将从传统及新型血清肿瘤标志物、内镜检查及基因水平三个方面对胃癌的诊断进展予以综述。

血清结肠癌转移相关基因-1在晚期胃癌组织中的表达及对阿帕替尼化疗疗效的预测价值

目的探究血清结肠癌转移相关基因-1(MACC1蛋白)在晚期胃癌组织中的表达及对阿帕替尼化疗疗效的预测价值。方法选取60例晚期胃癌患者,按治疗方法的不同将其分为对照组(n=36)和观察组(n=24)。对照组给予替吉奥片、奥沙利铂甘露醇注射液治疗,观察组在此基础上加用阿帕替尼片,所有患者均化疗3个周期。统计MACC1蛋白在正常胃黏膜组织和胃癌组织中的表达情况;统计化疗前和化疗3个周期后2组患者MACC1蛋白含量,统计2组患者化疗3个周期后的预后情况。结果MACC1蛋白在胃癌组织中的阳性表达率显著高于正常胃黏膜组织中的表达率;化疗3个周期后,2组患者的MACC1蛋白含量均降低,且观察组较对照组降低的更显著,观察组的无进展生存时间和总生存时间均显著长于对照组(P<0.01)。结论MACC1有助于胃癌的诊断,且MACC1越低阿帕替尼的化疗效果越好。

阿帕替尼联合替吉奥治疗晚期胃癌的临床疗效及对血清MMP-2、REGⅣ和SRF水平的影响

目的:探讨阿帕替尼联合替吉奥(tegio,S-1)治疗晚期胃癌的临床疗效及对血清基质金属蛋白酶-2(matrix metalloproteinase-2,MMP-2)、再生基因蛋白Ⅳ(regenerated gene proteinⅣ,REGⅣ)和反应因子(serum response factor,SRF)水平的影响。方法:选取2017年01月至2018年04月在我院治疗的晚期胃癌患者107例,根据治疗方案分为观察组(n=49)和对照组(n=58),观察组给予阿帕替尼联合S-1治疗,对照组给予S-1治疗,观察两组患者治疗疗效、生存时间、不良反应等,检测血清MMP-2、REGⅣ和SRF水平。结果:观察组患者治疗疗效优于对照组(P<0.05),其治疗总有效率为69.39%;观察组患者治疗后血清MMP-2、REGⅣ和SRF分别为(3454.49±283.39)ng/L、(2.01±0.72)ng/L和(33.38±9.28)ng/mL,明显低于对照组(P<0.05);观察组患者中位生存时间为19.00个月,明显长于对照组(P<0.05);观察组和对照组患者不良反应发生率比较,差异无统计学意义(P>0.05)。结论:阿帕替尼联合S-1治疗晚期胃癌有较好的临床疗效,可明显降低血清MMP-2、REGⅣ和SRF水平。

胃癌患者血清中抑癌基因超甲基化检测的临床意义分析

目的:探讨胃癌患者血清中抑癌基因超甲基化检测的临床意义。方法:收集于2019年1月2019年12月在我院检测的高危胃癌患者78例进行研究,其中21例胃癌患者为A组,29例萎缩性胃炎为B组,28例健康者为对照组。分别检测各组的CDKN2A、CDH1、DAPK1抑癌基因的甲基化水平。以病理诊断作为金标准,比较血清中抑癌基因超甲基化的阳性率及诊断敏感性、特异性。结果:A组CDKN2A、CDH1、DAPK1基因启动子甲基化的阳性率明显高于B组和对照组,差异有统计学意义(P<0.05)。联合检测的诊断灵敏度、特异性明显高于单独检测。结论:联合检测血清CDKN2A、CDH1、DAPK1抑癌基因甲基化水平对胃癌疾病诊断的灵敏度及特异性较高,可作为胃癌疾病评估的标志物。

血清胃蛋白酶原与再生基因Ⅳ联合检验对胃癌早期诊断价值

目的分析血清胃蛋白酶原(PG)与再生基因Ⅳ(RegⅣ)联合检验对胃癌早期诊断价值。方法随机选择2019年2月—2020年2月该院收治胃病患者50例,依据病理诊断结果分成两组,胃癌组20例,良性胃病组30例,另选择同期行健康体检者50名为对照组,对各组血清CEA、PG、CA19-9、RegⅣ水平进行比较,对比PG与RegⅣ联合检验诊断结果。结果胃癌组血清的PGI(41.85±11.51)μg/L、PGⅡ(8.50±3.38)μg/L、PGI/PGⅡ(2.53±1.08)指标比良性胃病组与对照组低,差异有统计学意义(P<0.05);良性胃病组血清的PGI、PGⅡ、PGI/PGⅡ指标比对照组高,差异有统计学意义(P<0.05);胃癌组血清的RegⅣ、CEA、CA19-9指标比良性胃病组与对照组高,差异有统计学意义(P<0.05);良性胃病组血清的RegⅣ、CEA、CA19-9指标比对照组高,差异有统计学意义(P<0.05);PG联合RegⅣ检验敏感度为70.00%、特异性为53.33%,高于CA19-9联合CEA检验,差异有统计学意义(P<0.05)。结论临床采用PG联合RegⅣ检验方式诊断胃癌,对胃癌具较高的特异性及灵敏度,可为临床诊治提供有效依据。

加味四君子汤含药血清对胃癌细胞SGC-7901凋亡相关因子表达的影响

目的:研究加味四君子汤含药血清对胃癌细胞SGC-7901凋亡相关因子表达的影响,进一步探讨其具体抗肿瘤作用机制。方法:40只SD大鼠随机分为加味四君子汤低、中、高剂量组(0.213,0.426,0.853 g·kg^(-1)),空白组,每组10只,空白组给予等体积的生理盐水灌胃,各组连续灌胃10 d,末次给药1.5 h后,水合氯醛腹腔麻醉,心脏采血,分离血清,56℃灭菌,0.22μm过滤,制备加味四君子汤高、中、低剂量组含药血清,各剂量组含药血清孵育胃癌细胞SGC-7901,运用流式细胞仪检测细胞早期和晚期凋亡情况,运用实时荧光定量聚合酶链式反应(Real-time PCR)技术检测肿瘤抑制基因p53,c-核蛋白类基因(c-Myc),半胱氨酸天冬氨酸蛋白酶-3(Caspase-3),凋亡相关基因B细胞淋巴瘤-2(Bcl-2)mRNA的表达,运用细胞免疫荧光技术检测p53,c-Myc,Caspase-3,Bcl-2蛋白的相对表达量情况。结果:与空白组比较,加味四君子汤含药血清高剂量组细胞凋亡比率显著升高(P<0.01),且可使胃癌细胞SGC-7901早期+晚期凋亡率达到22.58%(P<0.01)。Real-time PCR结果显示加味四君子汤中剂量组能显著促进Caspase-3 mRNA表达(P<0.01),加味四君子汤高剂量组能显著上调p53及c-Myc mRNA表达量(P<0.01),加味四君子汤高剂量组显著抑制Bcl-2 mRNA表达(P<0.01)。免疫荧光结果显示加味加味四君子汤高剂量组能使c-Myc,Caspase-3,p53蛋白表达水平显著升高(P<0.01),而Bcl-2蛋白表达水平显著降低(P<0.05)。结论:加味四君子汤含药血清能抑制抗凋亡蛋白Bcl-2的表达,促进凋亡相关分子p53,c-Myc,Caspase-3的表达,发挥抗肿瘤作用。