O6-methylguanine DNA methyltransferase is upregulated in malignant transformation of gastric epithelial cells via its gene promoter DNA hypomethylation

BACKGROUND O_(6)-methylguanine-DNA methyltransferase(MGMT)is a suicide enzyme that repairs the mispairing base O_(6)-methyl-guanine induced by environmental and experimental carcinogens.It can transfer the alkyl group to a cysteine residue in its active site and became inactive.The chemical carcinogen N-nitroso compounds(NOCs)can directly bind to the DNA and induce the O_(6)-methylguanine adducts,which is an important cause of gene mutation and tumorigenesis.However,the underlying regulatory mechanism of MGMT involved in NOCs-induced tumorigenesis,especially in the initiation phase,remains largely unclear.AIM To investigate the molecular regulatory mechanism of MGMT in NOCs-induced gastric cell malignant transformation and tumorigenesis.METHODS We established a gastric epithelial cell malignant transformation model induced by N-methyl-N’-nitro-N-nitrosoguanidine(MNNG)or N-methyl-N-nitroso-urea(MNU)treatment.Cell proliferation,colony formation,soft agar,cell migration,and xenograft assays were used to verify the malignant phenotype.By using quantitative real-time polymerase chain reaction(qPCR)and Western blot analysis,we detected the MGMT expression in malignant transformed cells.We also confirmed the MGMT expression in early stage gastric tumor tissues by qPCR and immunohistochemistry.MGMT gene promoter DNA methylation level was analyzed by methylation-specific PCR and bisulfite sequencing PCR.The role of MGMT in cell malignant transformation was analyzed by colony formation and soft agar assays.RESULTS We observed a constant increase in MGMT mRNA and protein expression in gastric epithelial cell malignant transformation induced by MNNG or MNU treatment.Moreover,we found a reduction of MGMT gene promoter methylation level by methylation-specific PCR and bisulfite sequencing PCR in MNNG/MNU-treated cells.Inhibition of the MGMT expression by O_(6)-benzylguanine promoted the MNNG/MNU-induced malignant phenotypes.Overexpression of MGMT partially reversed the cell malignant transformation process induced by MNNG/MNU.Clinical gastric tissue analysis showed that MGMT was upregulated in the precancerous lesions and metaplasia tissues,but downregulated in the gastric cancer tissues.CONCLUSION Our finding indicated that MGMT upregulation is induced via its DNA promoter hypomethylation.The highly expressed MGMT prevents the NOCs-induced cell malignant transformation and tumorigenesis,which suggests a potential novel approach for chemical carcinogenesis intervention by regulating aberrant epigenetic mechanisms.

薄皮甜瓜9-脂氧合酶(9-LOX)类型的CmLOX09对逆境、激素和信号类物质的响应（英文）

目的:研究CmLOX09及其下游基因CmHPL和Cm AOS对逆境、激素和信号类物质的响应,进一步测定茉莉酸甲酯(Me JA)处理后叶片中绿叶挥发物的含量以及接种白粉病菌后叶片中茉莉酸含量的变化,探讨脂氧合酶(LOX)响应这两种胁迫的可能途径。创新点:通过对CmLOX09启动子中顺式作用原件的分析预测,首次研究薄皮甜瓜9-LOX类型的CmLOX09对机械损伤、激素、信号类物质以及生物胁迫的响应。方法:利用Plant CARE软件对Cm LOX09启动子响应元件进行预测分析(图S1);利用荧光定量聚合酶链反应(q RT-PCR)技术分析甜瓜在机械损伤、激素、信号类物质以及生物胁迫处理后叶片中CmLOX09、CmHPL和CmAOS的表达模式;利用气相色谱-质谱连用仪(GC-MS)测定叶片中绿叶挥发物的含量(图4);利用高效液相色谱-串联质谱法(HPLC-MS/MS)分析和测定叶片中茉莉酸的含量(图6)。结论:本研究结果显示:CmLOX09参与机械损伤、激素、信号类物质及白粉病菌的防御反应(图1~3,5)。9-LOX类型的CmLOX09可能通过氢过氧化物裂解酶(HPL)途径产生的绿叶挥发物(GLV)来响应Me JA(图4),并通过丙二烯合酶(AOS)途径产生的茉莉酸来响应真菌胁迫(图6)。综上所述,9-LOX类型的CmLOX09可能在生物和非生物胁迫反应中起重要作用。

多胺诱导产生的一氧化氮通过影响番茄幼苗抗氧化系统抵御低温胁迫（英文）

目的:研究多胺(PA)对低温胁迫下番茄幼苗中一氧化氮(NO)产生的影响,并探讨NO在PA诱导的耐冷性中发挥的作用。创新点:在番茄幼苗中证明亚精胺(Spd)对NO产生的影响及可能的作用途径,且此作用与番茄耐低温性有密切关系。方法:通过检测氧合血红蛋白(HbO 2)向高铁血红蛋白(met Hb)的转化进行NO含量测定;通过与NO特异性荧光探针(DAF-FM DA)结合检测NO释放量(图1和2)。超氧化物歧化酶(SOD)活性根据其抑制氮蓝四唑(NBT)在光下的还原作用测定;过氧化物酶(POD)活性通过测定酶提取液与愈创木酚、过氧化氢(H_2O_2)的混合物的吸光度确定;过氧化氢酶(CAT)活性根据H_2O_2在240 nm波长下的降解能力来测定;抗坏血酸过氧化物酶(APX)活性的测定参照Nakano和Asada(1981)的方法在波长290 nm下测定(图6和7)。结论:本研究的结果显示,Spd诱导番茄叶片中NO的产生可直接通过增加一氧化氮合酶(NOS)和硝酸还原酶(NR)的活性实现(图2)。H_2O_2作为上游信号能够刺激NO的生成(图3)。NO通过增加抗氧化酶活性和相关基因的表达来参与Spd诱导的番茄耐冷性(图6和7)。综上所述,Spd诱导产生的NO在番茄响应低温胁迫中发挥重要作用。