Amplification and function analysis of N6-adenine-specific DNA methyltransferase gene in Nilaparvata lugens

Methylation of the N6 position of adenine, termed N6-methyladenine, protects DNA from restriction endonucleases via the host-specific restriction-modification system. N6-methyladenine was discovered and has been well studied in bacteria. N6-adenine-specific DNA methyltransferase（N6AMT） is the main enzyme catalyzing the methylation of the adenine base and knowledge of this enzyme was mainly derived from work in prokaryotic models. However, large-scale gene discovery at the genome level in many model organisms indicated that the N6AMT gene also exists in eukaryotes, such as humans, mice, fruit flies and plants. Here, we cloned a N6AMT gene from Nilaparvata lugens（Nlu-N6AMT） and amplified its fulllength transcript. Then, we carried out a systematic investigation of N6AMT in 33 publically available insect genomes, indicating that all studied insects had N6AMT. Genomic structure analysis showed that insect N6AMT has short introns compared with the mammalian homologs. Domain and phylogenetic analysis indicated that insect N6AMT had a conserved N6-adenine Mlase domain that is specific to catalyze the adenine methylation. Nlu-N6AMT was highly expressed in the adult female. We knocked down Nlu-N6AMT by feeding ds RNA from the second instar nymph to adult female, inducing retard development of adult female. In all, we provide the first genome-wide analysis of N6AMT in insects and presented the experimental evidence that N6AMT might have important functions in reproductive development and ovary maturation.

O^6-甲基鸟嘌呤-DNA-甲基转移酶基因表达与胃癌发生的关系

目的研究人胃癌组织O6-甲基鸟嘌呤-DNA-甲基转移酶(MGMT)基因的表达特点及其与胃癌发生的关系。方法应用加强型原位杂交方法及寡核苷酸探针高效标记技术对76例胃癌组织、73例癌旁组织、20例正常胃组织进行MGMT基因标记检测,同时应用自动图像分析系统进行定量分析。结果胃癌组织MGMT基因阳性表达率为40.8%(31/76),低于正常胃组织的60.0%(12/20),MGMT表达强阳性率为32.3%(10/31),也明显低于正常组织的83.3%(10/12),差异均有显著性意义(P<0.01或P<0.05);癌旁组织MGMT基因阳性表达率为46.6%(34/73),MG-MT表达强阳性率为41.1%(14/34),与胃癌组织差异无显著性意义。定量分析示,胃癌组织MGMT阳性表达的积分吸光度、阳性单位值明显低于正常组织(P<0.05)。胃癌组织与癌旁组织、早期胃癌与进展期胃癌组织、癌旁不同程度不典型增生之间MGMT表达无明显差异。结论人体胃组织存在高度表达的MGMT基因,胃癌发生与MGMT基因表达水平降低有关,MGMT基因异常表达是胃癌形态学改变出现之前的早期行为。

O^6-甲基鸟嘌呤-DNA甲基转移酶基因多态性与胃癌遗传易感性的关系

目的探讨O6-甲基鸟嘌呤-DNA甲基转移酶(MGMT)基因第3外显子上第84和第53密码子上的多态性改变与胃癌易感性的关系以及与环境因素在胃癌发生中的交互作用。方法应用以人群为基础的病例对照研究,采用PCR-RFLP技术检测191例胃癌病例组与251例健康对照组MGMT-Leu53Leu和MGMT-Leu84Phe多态改变的频率。结果MGMT-Leu84Phe各基因型在胃癌病例组(CC 74.3%,CT 23.6%,TT 2.1%)和对照组(CC 74.1%,CT 23.5%,TT 2.4%)的分布情况与MGMT-Leu53Leu基因型相似,差异无显著性;MGMT-Leu53Leu各基因型在胃癌病例组中的分布分别为CC型(75.4%)、CT型(21.5%)、TT型(3.1%),对照组分布为CC型(72.1%)、CT型(24.7%)、TT型(3.2%),两组比较差异无显著性;分别按年龄、性别、吸烟、饮酒、H.pylori感染以及胃癌家族史等因素分层分析也没有发现两个位点的突变基因型与胃癌遗传易感性的相关性。结论结果显示MGMT-Leu53Leu、Leu84Phe与胃癌的发生没有显著关联。

O^6-methylguanine-DNA methyltransferase gene expression confers alkylation resistance to tumor cells

The emergence of drug resistance is a major obstacle limiting the successful chemotherapy of malignant tumors. Our previous studies have demonstrated that O^6-methylguanine-DNA methyltransferase (MGMT, EC 2.1.1.63) is an important contributor to tumor cellular resistance toward mono- and bifunctional alkylating agents, such as 1- (4-amino-2-methyl-5-pyrimidinyl) methyl-3- (2-chloroethyl) -3-nitrosourea (ACNU) and N-methyl-N’-nitro-N-nitrosoguanidine (MNNG). Mechanistically, MGMT can specifically remove the induced alkyl groups at the O^6-position of guanine which finally would lead to a G→ A transition or a lethal DNA interstrand cross-link unless repaired. Cells

Protective effect of O^6-methylguanine-DNA-methyltransferase on mammalian cells

Background O^6-methylguanine-DNA-methyltransferase （MGMT） is a specific DNA revising enzyme transferring alkylated groups from DNA to its cysteine residue to avoid the abnormal twisting of DNA. Therefore, it is one of the drug resistant genes targeted in the treatment of cancer. This study explored the protective effect of MGMT gene transferred into mammalian cells. Methods Mammalian expression vector containing the MGMT gene cloned from human hepatocytes by RT-PCR was constructed and transferred into K562 cells and human peripheral blood mononuclear cells （PBMCs） via liposome, then assayed for gene expression at RNA and protein levels. MIF assay was used to check the drug resistance of cells transfected with MGMT gene. Results MGMT gene was successfully cloned. Real-time PCR showed that the mRNA expression in gene transfected groups in K562 cell line and PBMC were 13.4 and 4.0 times that of the empty vector transfected groups respectively. Results of Western blotting showed distinct higher expression of MGMT in gene transfected group than in other two groups. The IC50 values increased to 7 and 2 times that of the original values respectively in stable transfected K562 cells and transient transfected PBMC. Conclusion The alkylating resistance of eukaryotic cells is enhanced after being transfected with MGMT gene which protein product performs the protective function, and may provide the reference for the protective model of peripheral blood cells in cancer chemotherapy.

G156A六氧甲基鸟嘌呤-DNA-甲基转移酶原核表达载体的构建和表达

目的 :构建原核表达载体pPROEXHTb G15 6AMGMT ,观察突变型G15 6AMGMT在大肠杆菌中的表达情况。方法 :通过基因重组技术将G15 6AMGMT亚克隆至pPROEXHTb原核表达载体 ,在大肠杆菌DH5α中经异丙基硫代 β D半乳糖苷 (IPTG)诱导表达。 结果 :经PCR及酶切分析证实 ,成功构建了pPROEXHTb G15 6AMGMT原核表达载体 ,经SDS 聚丙烯酰胺凝胶电泳 (SDS PAGE)显示重组克隆化基因pPROEXHTb G15 6AMGMT在大肠杆菌DH5α中有表达。结论 :G15 6AMGMT在大肠杆菌DH5α中有表达 ,为获取突变型MGMT工程蛋白奠定了基础。

Promoter Hypermethylation of DNA Repair Gene MGMT in Laryngeal Squamous Cell Carcinoma

The relationship between hypermethylation of CpG islands in the promoter regions of O^6- methylguanine DNA methyhransferase （MGMT） genes and laryngeal squamous cell carcinoma was explored. Methylation-specific PCR and semi-quantitative RT-PCR were used to study the promoter methylation and mRNA expression of the MGMT gene in laryngeal carcinoma tissues, tissues adjacent to the tumor and normal laryngeal tissues. Hypermethylation of MGMT gene was detected in 16 samples of 46 （34.8 %） laryngeal squamous cell carcinoma samples. However, the MGMT hypermethylation was not detected in all tissues adjacent to the tumors and normal tissues. No significant difference in MGMT gene hypermethylation was found in samples with different histological grades （χ^2= 3. 130, P=0. 077） or in samples from patients with different TNM status （χ^2= 3. 957, P=0. 138）. No expression of MGMT mRNA was detected in all hypermethylated laryngeal carcinoma tissues. The expression of MGMT mRNA was detected in all unmethylated laryngeal carcinoma tissues, tissues adjacent to the tumors and normal tissues. It suggests that MGMT gene promoter hypermethylation is associated with MGMT gene transcription loss in laryngeal carcinoma tissues and possibly plays an important role in carcinogenesis of laryngeal tissues.

Promoter methylation status of hMLH1,MGMT,and CDKN2A/p16 in colorectal adenomas

AIM:To investigate aberrant DNA methylation of CpG islands and subsequent low-or high-level DNA microsatellite instability(MSI)which is assumed to drive colon carcinogenesis. METHODS:DNA of healthy individuals,adenoma(tu-bular or villous/tubulovillous)patients,and colorectal carcinoma patients who underwent colonoscopy was used for assessing the prevalence of aberrant DNA methylation of human DNA mismatch repair gene mutator L homologue 1(hMLH1),Cyclin-dependent kinase inhibitor 2A(CDKN2A/p16),and O-6-methylguanine DNA methyltransferase(MGMT),as well as their rela- tion to MSI. RESULTS:The frequency of promoter methylation for each locus increased in the sequence healthy tissue/adenoma/carcinoma.MGMT showed the highest frequency in each group.MGMT and CDKN2A/p16 presented a statistically significant increase in promoter methylation between the less and more tumorigenic forms of colorectal adenomas(tubular vs tubullovillous and villous adenomas).All patients with tubulovillous/villous adenomas,as well as all colorectal cancer patients,showed promoter methylation in at least one of the examined loci.These findings suggest a potentially crucial role for methylation in the polyp/adenoma to cancer progres- sion in colorectal carcinogenesis.MSI and methylation seem to be interdependent,as simultaneous hMLH1, CDKN2A/p16,and MGMT promoter methylation was present in 8/9 colorectal cancer patients showing the MSI phenotype. CONCLUSION:Methylation analysis of hMLH1,CD- KN2A/p16,and MGMT revealed specific methylation profiles for tubular adenomas,tubulovillous/villous adenomas,and colorectal cancers,supporting the use of these alterations in assessment of colorectal tumorigenesis.

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、hMLH1和hMSH2基因启动子甲基化状态对脑胶质瘤预后的影响

目的探讨脑胶质瘤DNA修复基因O6-甲基鸟嘌呤-DNA甲基转移酶(MGMT)和错配修复基因(MMR)(hMLH1、hMSH2)启动子甲基化状态及其对患者预后和烷化剂化疗敏感性的影响。方法采用甲基化特异性PCR(MSP)方法检测39例脑胶质瘤和6例正常脑组织MGMT、hMLH1和hMSH2基因启动子区的甲基化状态,免疫组化方法测定其蛋白表达。绘制Kaplan-merier生存曲线。结果脑胶质瘤组织MGMT、hMLH1和hMSH2基因启动子区甲基化发生率分别为46.2%、10.3%和20.5%,而正常脑组织相应基因启动子区未发生甲基化;三种基因启动子未甲基化模式与其对应蛋白表达模式相似。MGMT基因甲基化的脑胶质瘤患者存活率显著高于未甲基化者(P<0.05);MMR基因甲基化患者中MGMT基因甲基化与未甲基化者的生存期无统计学差异(P>0.05)。结论hMLH1、hMSH2及MGMT甲基化是脑胶质瘤发生过程中常见的分子事件;联合检测MGMT、hMLH1和hM-SH2基因启动子甲基化状态可判断脑胶质瘤患者的预后及其对烷化剂化疗的敏感性。

胃癌组织中MDR和MGMT基因表达及其相关意义

目的:检测胃癌组织多药耐药(multidrugresistance,MDR)基因和O6-甲基鸟嘌呤-DNA-甲基转移酶(O6-methylguanin-e-DNA-meyhyltransferase,MGMT)基因的表达,探讨MDR、MGMT基因表达的相关性及其在胃癌组织中的临床病理学意义。方法:应用加强型原位杂交技术通过核酸探针对76例胃癌组织进行MDR、MGMT基因检测,同时应用自动图像分析系统进行定量分析。结果:76例胃癌组织中MDR基因阳性表达率为68·4%,积分吸光度为351·5±121·4,分别高于正常组织(40·0%,168·4±68·8);MGMT阳性表达率为40·8%,积分吸光度为161·4±78·84,分别低于正常组织(60·4%,332·9±118·2)。生存时间5年以下组MDR和MGMT基因表达分别高于5年以上组,rs分别为0·250和0·287,P值分别为0·010和0·008;白细胞计数>3×109L-1组MGMT基因表达高于<3×109L-1组,rs=0·354,P=0·001;有淋巴结转移组MDR基因表达高于无淋巴结转移组,rs=0·280,P=0·004;术前化疗组MDR表达明显高于未化疗组,rs=0·300,P=0·002。结论:胃癌组织存在原发性和获得性MDR基因耐药的双重性,而MGMT基因主要是原发性,两种基因表达可能是2个相互独立的事件,在胃癌预后和骨髓抑制的判断上有一定意义。

燃煤污染型地方性氟中毒患者血细胞hMLH1与MGMT mRNA表达改变

目的探讨燃煤污染型地方性氟中毒(简称燃煤型地氟病)对血液中错配修复基因(hMLH1)及O(6)-甲基鸟嘌呤DNA甲基转移酶基因(MGMT)mRNA表达水平的影响。方法在贵州省毕节地区燃煤型地氟病区抽取45例患者,按其氟斑牙和氟骨症严重程度分为轻、中、重度组各15例。在毕节地区非病区抽取15名村民作为对照组。实时荧光定量PCR技术检测各组血样本MGMT、hMLH1mRNA水平。结果燃煤型氟中毒轻、中、重度3个组中hMLH1及MGMT mRNA水平与对照组相比明显降低,差异有统计学意义(P<0.05),且随着氟中毒程度的加重,其降低程度更加明显。组间两两比较,随着中毒程度加重,表达水平明显降低(P<0.05)。结论 MGMT与hMLH1mRNA水平在燃煤型氟中毒所造成的DNA损伤及修复机制中可能有负面作用。

反义RNA调节MGMT基因表达逆转肿瘤细胞对嘧啶亚硝脲的耐药性

目的：抑制细胞内的Ｏ６－甲基鸟嘌呤－ＤＮＡ甲基转移酶（ＭＧＭＴ）基因表达水平，逆转肿瘤细胞对嘧啶亚硝脲的耐药性。方法：本实验构建了三个表达ＭＧＭＴ反义ＲＮＡ的逆转录病毒载体（ｐＬＭＴＳＮＡＳ，ｐＬＭ５ＳＮＡＳ和ｐＬＭ３ＳＮＡＳ），并用它们转导ＨｅＬａＳ３肿瘤细胞，观察细胞在转导前后ＭＧＭＴ基因表达水平及其对嘧啶亚硝脲（ＡＣＮＵ）抗药性的变化。结果：研究发现针对ＭＧＭＴｍＲＮＡ５端的反义ＲＮＡ能够有效地降低ＨｅＬａＳ３细胞的ＭＧＭＴ基因表达水平（为对照细胞的３０％～４０％），并使细胞对ＡＣＮＵ的敏感性提高４．６倍；针对ＭＧＭＴｍＲＮＡ全长的反义ＲＮＡ，也能在一定程度上调节细胞的ＭＧＭＴ基因表达水平并增加细胞对ＡＣＮＵ的敏感性，而针对３端序列的反义ＲＮＡ对ＭＧＭＴ基因无调节作用。转导细胞对ＡＣＮＵ耐药性的变化与ＭＧＭＴ基因表达水平的抑制程度密切相关。结论：合适的反义ＲＮＡ能够有效地调节ＭＧＭＴ基因表达水平。

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.

DNA修复蛋白MGMT基因的克隆及转导脐血CD34^+细胞后耐药特征的研究

目的 增强脐血 CD34+造血细胞对化疗药物的耐药表型 ,探讨逆转录病毒介导的基因转移效率和耐药基因特性 ,以及在脐血造血干细胞保护性基因治疗中的作用和意义。方法 应用逆转录 -聚合酶链反应 (RT- PCR)从人肝组织中获得编码六氧甲基鸟嘌呤 - DNA-甲基转移酶 (O6 - methylguanine- DNA-methyltransferase,MGMT) c DNA;利用基因重组技术 ,将其克隆于 p GEM- T质粒载体并构建了逆转录病毒载体 G1Na- MGMT;应用脂质体 L ipofect AMINE基因转移法将后者导入 GP+ E86和 PA317病毒包装细胞 ,以卡氮芥 1,3- Bis(2 - Chloroethyl) - 1- Nitrosourea(BCNU)加压筛选后的阳性克隆上清经乒乓效应后继而感染脐血 CD34+ 细胞。应用 PCR,Southern Blot,RT- PCR,Northern blot,Western Blot及 MTT法检测 MGMT基因在脐血 CD34+ 细胞中的转移和表达。结果 酶切鉴定及 DNA测序证实了 MGMT c DNA克隆的正确性 ,脂质体介导方法成功将其导入病毒包装细胞 ,BCNU加压筛选和乒乓感染法使病毒效价达1.6× 10 6 CFU/ml,逆转录病毒载体介导的 MGMT基因在脐血造血干细胞中获得了有效转移和表达。转MGMT耐药基因脐血造血干 /祖细胞对 BCNU的抗药性较对照组提高了 4倍。结论 DNA修复蛋白MGMT基因的克隆并导入脐血造血干 /祖细胞可?

亚砷酸钠对HaCaT细胞MGMT基因启动子区甲基化CpG结合蛋白-2、DNA甲基转移酶1、组蛋白去乙酰化酶-1结合的影响

目的观察亚砷酸钠（NaAsO：）对人肤角质形成细胞株（HaCaT细胞）MGMT基因启动子区甲基化CpG结合蛋白-2（MeCP2）、DNA甲基转移酶1（DNMTl）及组蛋白去乙酰化酶1（HDACl）结合情况的影响，为深化阐释砷毒作用机制提供依据。方法分别以0．00（空白对照）、3．13、6，25、12．50、25．00μmol／LNaAs02重复间隔处理HaCaT细胞72h（NaAs02处理24h，隔天再次相同处理，重复3次），以人表皮鳞癌细胞株（A431）作为阳性对照。定量染色质免疫共沉淀技术（Q—CHIP）检测MGMT基因转录调控区CHIPl、CHIP2区域及MGMT基因编码区ChIP3区域MeCP2、DNMTl、HDACl结合情况。结果各组HaCaT细胞MGMT基因转录调控区CHIPl、CHIP2区域MeCP2、DNMTl、HDACl蛋白结合水平比较，差异有统计学意义（F值分别为7．387、84．634、78．442和19．263、69．649、26．546，P均〈0．05）；其中各N以s02处理组CHIPl、CHIP2区域MeCI〉2、DNMTl、HDACl蛋白结合水平[3．13μmol／LNaAs02处理组：（136．00±16．97）％、（145．00±2．83）％、（88．50±19．09）％和（106．50±37．48）％、（112．34±8．73）％、（59．71±8．49）％；6．25μmol／LNaAs02处理组：（130．00±42．43）％、（154．50士4．95）％、（101．00±1．27）％和（88．50±3．54）％、（134．32±2．82）％、（102．75±19．91）％；12．50~mol／LNaAs02处理组：（141．50±23．33）％、（161．50±7．78）％、（125．00±U．31）％和（119．50±24．75）％、（171．59±3．54）％、（167．61±10．61）％；25，00μmol／LNaAs02处理组：（134．50±43．13）％、（472．50±50．20）％、（383．50±30．41）％和（180．09±12．73）％、（348．50±27．58）％、（158．45±12．02）％]均高于空白对照组[（51．50±9．19）％、（82．00±12．73）％、（25．03±2．91）％和（37．02±4．24）％、（91．56±26．16）％、（19．09±2．90）％，P均〈0．05]。各组HaCaT细胞MGMT基因编码区CHIP3区域MeCP2蛋白结合水平比较，差异无统计学意义（F=1．670，P〉0．05），而DNMTl、HDACl蛋白结合水平比较，差异有统计学意义（F值分别为4．404、9．863，P均〈0．05），其中25．00I,Lmol／LNaAs02处理组DNMTl、HDACl蛋白结合水平[（615．85±29．63）％、（306．09±59．40）％]与空白对照组[（99．70±12．02）％、（92．45，±48．79）％]比较，差异有统计学意义（P均〈0．05）。结论MeCP2可结合于砷所致高甲基化MGMT基因转录调控区。通过招募DNMTl及HDACl使组蛋白去乙酰化，同时DNMTl可结合于MGMT基因编码区，以非甲基化DNA结合蛋白（IVIBD）依赖的方式招募HDACl，通过染色质重塑方式导致MGMT基因沉默，可能是砷毒性表现的早期分子事件。

森林草莓6mA甲基转移酶基因鉴定及功能分析

通过生物信息学手段,鉴定出森林草莓(Fragaria vesca)基因组中两类可能的6mA甲基转移酶基因5个(3个MT-A70、2个DAMT基因)。对细菌、真菌、动物和植物中的6mA甲基转移酶基因的系统进化分析及染色体定位表明,森林草莓MT-A70基因可分为3个亚家族,且在动、植物分化前就已经存在:两个DAMT基因由物种特异的串联重复产生,且结构变化快,推测其在进化历程中功能发生了分化。转录组数据及实时定量荧光PCR分析显示,各个基因均具有时空表达特异性和非生物胁迫响应。其中1个DAMT基因表达量在果实中较高且随果实成熟上调,推测可能参与调控果实成熟。此外,这5个基因在冷胁迫下表达水平有不同程度下调:而在热胁迫下各基因表达量变化显著不同。由此推测6m A甲基转移酶基因可能参与了森林草莓的生长发育和对冷、热胁迫的响应。

As3MT、N6AMT1基因-环境交互作用对砷暴露所致皮肤损伤影响

目的探讨砷甲基转移酶(As3MT)和N-6-腺嘌呤特异性DNA甲基转移酶1(N6AMT1)基因多态性及基因-环境交互作用与砷暴露所致皮肤损伤(AISL)的关联性。方法于2010年9月到2011年12月在内蒙古五原县入选饮水型砷暴露人群335人,65例被确诊患有AISL。应用MassARRAY^(?)分子量阵列平台检测基因型,高效液相色谱-电感耦合等离子体质谱联用法测定尿砷代谢物,砷暴露时间由其高砷水饮用时间确定,多因子降维法与岭回归模型分析基因型、环境因素的单独效应及基因-环境的交互作用。结果 As3MT基因rs3740400位点CA/AA基因型、N6AMT1基因rs 1006903位点GC/CC基因型和尿二甲基胂酸(DMA)升高为AISL的独立危险因素(P<0.05)。rs3740400位点基因型-尿无机砷(iAs)-单甲基胂酸(MMA)的交互作用与AISL发生风险间存在显著的统计学关联(OR=0.62, 95%CI=0.41～0.94,P=0.024),模型的验证样本准确率为0.577 6,交叉验证一致性为9/10。结论 As3MT、N6AMT1基因多态性及尿砷化合物水平均与AISL独立相关,rs3740400位点基因型、尿iAs和MMA的交互作用在慢性砷中毒的发生发展中具有重要作用。

燃煤污染型砷中毒人群MGMT基因甲基化、转录及表达的研究

目的了解O6-甲基鸟嘌呤DNA甲基转移酶基因(MGMT基因)启动子区甲基化、转录及表达以及DNA甲基转移酶1(DNMT1)的转录及表达与砷中毒的关系。方法采集68例燃煤污染型砷中毒(以下简称砷中毒)患者(轻度24例、中度28例、重度16例)及23例非病区居民外周血。用甲基化特异性PCR法(MSP)检测MGMT基因启动子区甲基化,实时荧光定量PCR(FQ-PCR)法检测MGMT及DNMT1 mRNA的水平。利用自愿手术治疗的砷中毒患者皮肤组织标本(61例,其中34例为一般病变,21例为癌前病变,6例为癌变)和对照皮肤组织标本(15例),以免疫组织化学(IHC)法检测砷中毒患者及对照皮肤组织中MGMT及DNMT1蛋白的表达。结果 MGMT基因启动子区甲基化阳性率与砷中毒程度有关(χ2=13.739,P<0.01)。砷中毒组MGMT mRNA表达水平与对照组比较,差异无统计学意义(P>0.05);MGMT基因启动子区甲基化患者和非甲基化患者之间MGMT mRNA和DNMT1 mRNA表达差异无统计学意义(P>0.05)。但轻、中度患者DNMT1 mRNA表达明显低于对照组(P<0.01);癌前病变组和癌变组皮肤组织中MGMT蛋白表达明显低于对照组(P<0.01),与皮肤损害程度有关(rs=-0.446,P<0.01);MGMT基因启动子区甲基化患者MGMT蛋白表达明显低于非甲基化组(P<0.05)。砷中毒组皮肤组织中DNMT1蛋白表达强于对照组(P<0.01),并与皮肤损害程度有关(rs=0.740,P<0.01);且MGMT基因启动子区甲基化患者组织中DNMT1蛋白表达明显高于非甲基化组(P<0.05)。结论 MGMT基因启动子区高甲基化抑制了燃煤污染型砷中毒患者皮肤组织中MGMT蛋白的表达,且DNMT1蛋白的高表达参与了此抑制过程。