Temozolomide and radiotherapy in newly diagnosed glioblastoma patients:O^6-methylguanine-DNA methyltransferase (MGMT) promotor methylation status and Ki-67 as biomarkers for survival and response to treatment

Objective:This phase II study aimed at investigating the correlation between O6-methylguanine-DNA methyltransferase (MGMT) promoter methylation and protein expression,together with Ki-67 labeling index (LI),to response,time to progression (TTP),and overall survival (OS) in newly diagnosed glioblastoma multiforme (GBM) patients treated with temozolomide (TMZ) concomitant with and adjuvant to radiotherapy (RT).Methods:From June 2005 to August 2008,34 adult patients (18-65 years),PS ≥70,with newly diagnosed GBM received TMZ 75 mg/m2 plus RT up to 60 Gy,followed by TMZ 175 mg/m2 5 days every 4 weeks for 12 doses.MGMT Methylation-specific PCR assay,MGMT protein expression,and Ki-67 expression using immunohistochemistry (IHC) were performed on the tissue blocks.The patients were followed by MRI while MR spectroscopy (MRS) was performed for the stable cases or to confirm progression and accordingly Bevacizumab 10 mg/kg every 2 weeks was added to 7 patients till further progression was proved.Results:31 cases were evaluable,12 (38.7%) had unmethylated MGMT,while 19 (61.3%) were methylated.Seventeen cases (55%) were MGMT immunonegative while 14 cases (45%) were immunopositive.The cut off value of Ki-67 LI in relation to survival was 17%,where 15 were < 17% (48.4%),and 16 were ≥ 17% (51.6%).Response evaluation started after the second dose of the adjuvant TMZ and was repeated every 2 months.The overall disease control rate (ODC) was 74.2%,where 2 patients had complete response (CR),14 had partial response (PR),and 7 had stable disease (SD),while 8 (25.8%) had progressive disease (PD).The ODC was significantly higher among methylated patients and in those with Ki-67 < 17% (P=0.0003).The median overall TTP was 12 months and the median OS was 20 months for all the patients including those who received Bevacizumab for some stable cases or as a salvage treatment in patients with good PS,the MGMT-methylated patients had a higher median TTP of 13 months (range 8 to 18 months,95% CI of 9.36 to 12.9),and OS of 24 months (range 12 to 31 months,95% CI of 16.1 to 21.32),while the unmethylated patients had a median TTP of 6.5 months and a median OS of 12 months,such correlations were highly significant (P=0.0001).MGMT immunoexpression failed to show significant correlation with MGMT promotor methylation or the outcome of the patients.Patients with Ki-67 < 17% had a median TTP of 16 months and median OS of 24 months compared to 7 and 12.5 months respectively for the patients with Ki-67 ≥17%.Significant correlation was found between the ODC,TTP,and OS with age < 52,near total excision,and TMZ doses received ≥ 10.The commonest grade 3 and 4 toxicities was neutropenia recorded in 3 patients (9.67%),thrombocytopenia in 4 patients (12.9%),and one patient with G3 nausea,vomiting,and constipations (3%),all were medically manageable.Conclusion:MGMT promotor methylation status and Ki-67 LI (but not the MGMT protein expression),could serve as prognostic markers for survival,also MGMT could identify the newly diagnosed GBM patients who will have better response to TMZ.

Expression of O⁶-Methylguanine-DNA Methyltransferase Examined by Alkyl-Transfer Assays, Methylation-Specific PCR and Western Blots in Tumors and Matched Normal Tissue

The tumor selectivity of alkylating agents that produce guanine O6-chloroethyl (laromustine and carmustine) and O6-methyl (temozolomide) lesions depends upon O6-methylguanine-DNA methyltransferase (MGMT) activity being lower in tumor than in host tissue. Despite the established role of MGMT as a tumor resistance factor, consensus on how to assess MGMT expression in clinical samples is unsettled. The aim of this study is to examine the relationship between the values derived from distinctive MGMT measurements in 13, 12, 6 and 2 pairs of human tumors and matched normal adjacent tissue from the colon, kidney, lung and liver, respectively, and in human cell lines. The MGMT measurements included 1) alkyl-transfer assays using [benzene-3H]O6-benzylguanine as a substrate to assess functional MGMT activity, 2) methylation-specific PCR (MSP) to probe MGMT gene promoter CpG methylations as a measure of gene silencing, and 3) western immunoblots to analyze the MGMT protein. In human cell lines, a strict negative correlation existed between MGMT activity and the extent of promoter methylation. In tissue specimens, by contrast, the correlation between these two variables was low. Moreover, alkyl-transfer assays identified 3 pairs of tumors and normal tissue with tumor-selective reduction in MGMT activity in the absence of promoter methylation. Cell line MGMT migrated as a single band in western analyses, whereas tissue MGMT was heterogeneous around its molecular size and at much higher molecular masses, indicative of multi-layered post-translational modifications. Malignancy is occasionally associated with a mobility shift in MGMT. Contrary to the prevalent expectation that MGMT expression is governed at the level of gene silencing, these data suggest that other mechanisms that can lead to tumorselective reduction in MGMT activity exist in human tissue.

O^6-甲基鸟嘌呤-DNA甲基转移酶在大肠癌中的表达及意义

目的:检测大肠癌组织中O6-甲基鸟嘌呤-DNA甲基转移酶(MGMT)的表达情况及其在肿瘤发生发展中的作用和临床意义。方法:采用SABC免疫组化法检测79例大肠癌标本中MGMT的表达情况。结果:大肠癌中MGMT阳性率为53.16%(42/79),其阳性表达与性别、癌细胞浸润深度无关(P>0.05),与患者年龄、淋巴结转移情况有关(P<0.05)。结论:检测MGMT的表达情况对于大肠癌恶性程度的判断及临床化疗方案的制定具有指导作用。

Role of MGMT as biomarker in colorectal cancer

O6-methylguanine DNA methyltransferase(MGMT) gene promoter methylation plays an important role in colorectal carcinogenesis, occurring in about 30%-40% of metastatic colorectal cancer. Its prognostic role has not been defined yet, but loss of expression of MGMT, which is secondary to gene promoter methylation, results in an interesting high response to alkylating agents such as dacarbazine and temozolomide. In a phase 2 study on heavily pre-treated patients with MGMT methylated metastatic colorectal cancer, temozolomide achieved about 30% of disease control rate. Activating mutations of RAS or BRAF genes as well as mismatch repair deficiency may represent mechanisms of resistance to alkylating agents, but a dose-dense schedule of temozolomide may potentially restore sensitivity in RAS-mutant patients. Further development of temozolomide in MGMT methylated colorectal cancer includes investigation of synergic combinations with other agents such as fluoropyrimidines and research for additional biomarkers, in order to better define the role of temozolomide in the treatment of individual patients.

MGMT is down-regulated independently of promoter DNA methylation in rats with all-trans retinoic acidinduced spina bifida aperta

O6-methylguanine DNA methyltransferase(MGMT), a DNA repair enzyme, has been reported in some congenital malformations, but it is less frequently reported in neural tube defects. This study investigated MGMT mRNA expression and methylation levels in the early embryo and in different embryonic stages, as well as the relationship between MGMT and neural tube defects. Spina bifida aperta was induced in rats by a single intragastric administration of all-trans retinoic acid on embryonic day(E) 10, whereas normal control rats received the same amount of olive oil on the same embryonic day. DNA damage was assessed by detecting γ-H2 A.X in spina bifida aperta rats. Real time-polymerase chain reaction was used to examine mRNA expression of MGMT in normal control and spina bifida aperta rats. In normal controls, the MGMT mRNA expression decreased with increasing embryonic days, and was remarkably reduced from E11 to E14, reaching a minimum at E18. In the spina bifida aperta model, γ-H2 A.X protein expression was increased, and mRNA expression of MGMT was markedly decreased on E14, E16, and E18. Bisulfite sequencing polymerase chain reaction for MGMT promoter methylation demonstrated that almost all CpG sites in the MGMT promoter remained unmethylated in both spina bifida aperta rats and normal controls, and there was no significant difference in methylation level between the two groups on either E14 or E18. Our results show that DNA damage occurs in spina bifida aperta rats. The mRNA expression of MGMT is downregulated, and this downregulation is independent of promoter DNA methylation.

MGMT基因启动子甲基化检测在脑胶质瘤化疗中的意义

背景与目的:如何预测和克服肿瘤细胞对化疗药物的耐药性,实施个体化治疗是肿瘤化疗急需解决的问题。与基因启动子甲基化密切相关的DNA损伤修复基因O6-甲基鸟嘌呤-DNA甲基转移酶(O6-methylguanine-DNA methyltransferase,MGMT)表观沉默与肿瘤对烷化剂药物化疗敏感性密切相关。本研究探讨检测MGMT基因启动子CpG岛甲基化在判断脑胶质瘤患者预后及预测肿瘤对烷化剂药物耐药性中的意义。方法:甲基化特异性PCR(MSP)法检测脑胶质瘤组织及肿瘤细胞株MGMT基因启动子甲基化状态,蛋白印迹和免疫组化法测定蛋白表达,MTT法检测肿瘤细胞株对烷化剂药物敏感性,将患者随访资料针对MGMT甲基化状态绘制Kaplan-Meier生存曲线,并进行log-rank检验分析。结果:39例脑胶质瘤患者组织MGMT基因启动子甲基化发生率为46.2%,蛋白表达阳性率为61.5%,且肿瘤组织中MGMT基因甲基化状态与蛋白表达显著相关(P<0.05);6例正常组织均未检测出基因甲基化。MGMT基因过甲基化的脑胶质瘤SHG-44细胞株用5-Aza-CdR处理后完全脱甲基化,MGMT蛋白恢复了表达,同时细胞株对烷化剂药物敏感性也发生逆转,由敏感转变为耐受。在采用手术、放疗和烷化剂尼莫司汀化疗等综合治疗的39例脑胶质瘤患者中,MGMT基因甲基化的患者生存率显著高于MGMT基因未甲基化患者(P<0.05)。结论:MGMT基因甲基化状态与蛋白表达及肿瘤细胞对烷化剂药物敏感性密切相关,有可能替代MGMT蛋白检测成为判断脑胶质瘤患者预后和预测肿瘤对烷化剂化疗耐药性的标志分子。

体外药敏实验及MGMT表达为依据的恶性脑胶质瘤个体化化疗:42例近期疗效分析

背景与目的:脑胶质瘤细胞对化疗药物耐药是导致化疗有效率低的重要原因之一。O6-甲基鸟嘌呤-DNA甲基转移酶(O6-methylguanine-DNAmethyltransferase,MGMT)可使DNA烷基化损伤得到修复,是细胞对治疗恶性脑胶质瘤的常用药物亚硝脲类及替莫唑胺(temozolomide,TMZ)产生耐药的主要原因。本研究采用体外药敏实验和检测肿瘤MGMT表达指导进行恶性脑胶质瘤个体化化疗,评价其近期疗效和不良反应。方法:经手术后病理确诊的恶性脑胶质瘤患者42例,取其新鲜肿瘤组织采用MTT法进行体外药敏实验,免疫组织化学方法检测肿瘤组织MGMT蛋白表达,根据体外药敏实验及MGMT测定结果选择化疗方案进行化疗。42例患者中有7例接受了2个方案化疗,共49例次可评价近期疗效。按WHO疗效评价标准进行近期疗效评价。不良反应评价按照美国国立癌症研究所评价标准。结果:6例次(12%)完全缓解,10例次(20%)部分缓解,20例次(41%)稳定,13例次(27%)进展。客观有效率为33%,疾病控制率为73%。80个周期可以评价不良反应,化疗的主要剂量限制性毒性为骨髓抑制,Ⅲ、Ⅳ级中性粒细胞减少占28%(22/80),Ⅳ级血红蛋白降低占1%(1/80),Ⅲ、Ⅳ级血小板减少占8%(6/80)。非血液学毒性主要为恶心/呕吐、脱发和疲劳。结论:根据体外药敏实验及MGMT蛋白表达选择化疗方案,对恶性脑胶质瘤患者进行个体化化疗,可以提高近期化疗疗效。

DNA修复酶(MGMT)在人胃肠癌中表达的临床意义

目的探讨MGMT在胃肠癌中表达的临床意义。方法93例胃肠癌(其中胃癌53例,大肠癌40例)利用SABC免疫组织化学方法检测MGMT。结果在胃肠癌中MGMT阳性率为49.46%(46/93),在胃癌和大肠癌中阳性率分别为45.28%(24/53)和55.00%(22/40)。66岁以上老年组MGMT阳性率明显低于其他年龄组(P<0.05),癌组织浸润深度达浆膜组和有淋巴结转移组MGMT阳性率高。MGMT在胃肠癌中的表达与性别和癌组织类型、分化程度相关性不明显(P>0.05)。结论MGMT在胃肠癌中的表达与年龄、浸润深度和淋巴结转移有关。

MGMT基因多态性与食管癌易感性关系

目的探讨山西省长治地区食管癌患者O6-甲基鸟嘌呤DNA甲基转移酶（MGMT）基因多态性与食管癌易感性的关系,及其与环境因素在食管癌发生中的交互作用。方法采用1∶1配对的病例对照研究,对201对研究对象进行食管癌相关危险因素的问卷调查,应用聚合酶链式反应-限制性片段长度多态性（PCR-RFLP）技术对MGMT多态性基因型进行检测。结果携带MGMT基因杂合型和突变型者发生食管癌的风险增高,χ2=9.80,P〈0.01,OR值分别为1.33（95%CI=1.01～2.07）和1.47（95%CI=1.03～2.54）;MGMT易感基因型与腌制食品对食管癌的发生存在交互作用（S=1.77,API=0.25）,而与吸烟、饮酒、精神刺激、食管癌家族史之间没有交互作用。结论MGMT突变基因型是长治地区食管癌高发的易感基因型,且与腌制食品存在协同作用。

卵巢癌组织中MGMT表达意义

目的探讨6-氧-甲基鸟嘌呤-DNA甲基转移酶(MGMT)在卵巢癌中的表达及临床意义。方法应用免疫组化(SP)法对60例卵巢癌及癌旁正常组织中MGMT的表达进行检测。结果60例卵巢癌组织中MGMT的表达率为46.7%,癌旁正常组织MGMT的表达率为100%(P<0.05)。MGMT的表达与卵巢癌的组织学类型和临床分期无关(P>0.05),但与卵巢癌的病理分级有关(P<0.05)。结论卵巢癌组织中存在MGMT的表达缺失,MGMT的功能失活可能是卵巢癌发生的重要机制之一。

干扰MGMT的人胶质瘤U251细胞对替莫唑胺的敏感性变化

目的观察干扰O6-甲基鸟嘌呤DNA甲基转移酶(MGMT)的人胶质瘤U251细胞对替莫唑胺(TMZ)的敏感性变化。方法培养人胶质瘤U251细胞,将U251细胞经16 mg/L替莫唑胺处理后分别转染si RNA-MGMT与siRNA-control,转染si RNA-MGMT质粒组为观察组,转染si RNA-control质粒组为对照组,不转染任何序列组为单药组,共培养48 h后收获细胞。qRT-PCR法检测三组细胞中MGMT的mRNA表达改变,MTT法观察各组U251细胞增殖能力,Transwell实验检测各组U251细胞侵袭能力。结果 qRT-PCR检测结果显示,观察组U251细胞中MGMT的mRNA表达量为(0.285±0.031),与对照组(1.104±0.096)和单药组(0.974±0.083)比较均明显下降,差异均有统计学意义(P<0.05),而对照组与单药组比较差异无统计学意义(P>0.05);MTT检测结果显示,观察组U251细胞的OD值为(0.392±0.014),与对照组(0.561±0.021)和单药组(0.530±0.019)比较均明显下降,差异均有统计学意义(P<0.05),而对照组与单药组比较差异无统计学意义(P>0.05);Transwell检测结果显示,观察组U251细胞穿过基质胶的数量为(64.27±7.04)个,与对照组[(128.14±14.37)个]和单药组[(119.63±10.92)个]比较均明显减少,差异均有统计学意义(P<0.05),而对照组与单药组比较差异无统计学意义(P>0.05)。结论干扰MGMT的人胶质瘤U251细胞对替莫唑胺的敏感性增强。

FHL2通过MGMT影响胶质母细胞瘤U87细胞对替莫唑胺的耐药性

目的:探讨干扰四个半LIM结构域蛋白2(FHL2)的表达对胶质母细胞瘤U87细胞中O6-甲基鸟嘌呤DNA甲基转移酶(MGMT)表达的影响,以及对U87细胞替莫唑胺(TMZ)耐药性的影响。方法:利用慢病毒感染技术分别将携带不同FHL2干扰序列的慢病毒(shFHL2-1#、shFHL2-4#)及其阴性对照(shN)感染U87细胞,分别命名为shFHL2-1#、shFHL2-4#和shN组;采用siRNA转染技术将siMGMT-1#、siMGMT-4#和siN转染至U87细胞,为siMGMT-1#、siMGMT-4#和siN组,qPCR和WB法验证FHL2或MGMT的敲低效果。用TMZ处理上述各组细胞(以DMSO处理组为对照),随后以CCK-8法和细胞克隆形成实验检测TMZ处理前后FHL2或MGMT敲低组细胞的增殖情况,FCM检测TMZ处理前后FHL2敲低组细胞的凋亡情况,WB法和免疫荧光法检测敲低FHL2对U87细胞中MGMT表达的影响,WB法检测TMZ处理对各组细胞中FHL2和MGMT表达水平的影响。结果:成功构建敲低FHL2或MGMT表达的U87细胞。与shN组相比,shFHL2-1#、shFHL2-4#组U87细胞的增殖能力减弱、凋亡水平升高(均P<0.01),MGMT表达水平明显降低(均P<0.01)。经TMZ处理后,与相应的DMSO处理组相比,shN组细胞中FHL2和MGMT的表达水平显著升高(均P<0.05),而细胞的增殖和凋亡均无显著变化(均P>0.05);shFHL2-1#、shFHL2-4#组细胞中FHL2和MGMT的表达水平无显著改变(均P>0.05),但细胞增殖能力进一步显著降低、凋亡水平进一步显著升高(均P<0.01)。敲低MGMT使U87细胞增殖减慢(P<0.01),而siMGMT-1#、siMGMT-4#组细胞经TMZ处理后增殖能力进一步降低(均P<0.01)。结论:干扰FHL2表达使得U87细胞增殖减慢而凋亡加剧、MGMT表达下调,提示FHL2可能通过影响MGMT的表达调控U87细胞对TMZ的耐药性。

维吾尔族妇女子宫颈鳞癌MGMT基因甲基化检测

目的检测O6-甲基鸟嘌呤-DNA甲基转移酶(O6-methylguanine-DNA methyltransferase,MGMT)基因启动子区甲基化与维吾尔族子宫颈鳞癌之间的相关性。方法采用甲基化特异性聚合酶链反应(methylation specific PCR,MSP)对41例维吾尔族妇女子宫颈鳞癌组织及32名正常维吾尔族妇女子宫颈组织进行甲基化检测。结果32名正常子宫颈组织MGMT基因启动子区均未发生甲基化,为非甲基化状态;41例子宫颈鳞癌组织中共有13例发生MGMT基因启动子区甲基化(32%)。结论MGMT基因启动子区甲基化可能部分参与维吾尔族妇女子宫颈癌的发生发展过程,是维吾尔族子宫颈鳞癌发生过程中常见的分子事件,有可能作为维吾尔族妇女子宫颈癌诊断的肿瘤标志物。

MGMT基因甲基化在肿瘤发生及个体性化疗中的意义

MGMT作为一种DNA修复蛋白,能够移除DNA上鸟嘌呤O6位点的能致突变毒性和细胞毒性的烷基加合物,从而保护细胞对抗烷化基团的损害,是肿瘤耐受烷化剂药物的主要原因。MGMT在不同的肿瘤和肿瘤细胞系中沉默,MGMT基因启动子CpG岛过甲基化是其表观沉默的主要机制。启动子过甲基化相关的MGMT基因沉默与很多人类肿瘤密切相关。首先,MGMT基因沉默可导致肿瘤相关基因转换突变的累积;其次,MGMT基因过甲基化与肿瘤增强对烷化剂药物敏感性之间呈正相关。这些新发现揭示了MGMT基因甲基化在肿瘤的发生、发展和肿瘤治疗中的重要作用。