过表达尿嘧啶DNA糖苷酶2(UNG2)可增强HepG2细胞的抗氧化作用

目的检测尿嘧啶DNA糖苷酶2(UNG2)的糖苷酶活性,研究UNG2在肝癌细胞HepG2抗氧化损伤过程中的作用。方法构建UNG2的过表达载体,利用Western blot法检测UNG2过表达效果。在HepG2细胞过表达UNG2,免疫荧光细胞化学染色观察UNG2在细胞中的表达和定位,利用含脱氧尿苷的寡核苷酸为底物测定UNG2的DNA糖苷酶活性,利用H_2O_2毒性实验研究UNG2在HepG2肝癌细胞抗氧化存活中的作用。结果在HEK293FT细胞中成功表达了UNG2,并发现UNG2主要定位在HepG2细胞核中。酶活性实验表明UNG2可以有效地切割寡核苷酸中的脱氧尿苷位点。H_2O_2毒性实验表明过表达UNG2可以显著提高HepG2肝癌细胞在H_2O_2处理后的存活率。结论 UNG2具有特异的尿嘧啶糖苷酶活性,并且UNG2能够保护HepG2肝癌细胞抵抗氧化应激损伤。

S期激酶相关蛋白2(SKP2)泛素化修饰OGG1对中波紫外线诱导的晶状体上皮细胞氧化损伤作用

目的探索E3泛素连接酶S期激酶相关蛋白2(SKP2)介导的碱基切除修复蛋白8-氧代鸟嘌呤-DNA糖基化酶(OGG1)在年龄相关性白内障(ARC)发生过程中的泛素化降解机制。方法采用免疫沉淀实验检测OGG1的泛素化修饰及其与SKP2的结合能力。采用中波紫外线(UVB)照射人晶状体上皮细胞株SRA01/04构建细胞氧化损伤模型。蛋白免疫印迹实验检测细胞氧化损伤模型和过表达模型细胞中SKP2的蛋白表达。通过转染SKP2质粒,增加SKP2的表达并观察细胞中OGG1蛋白的表达变化。结果OGG1蛋白存在泛素化修饰。UbiBrowser软件预测能与OGG1结合的潜在E3泛素连接酶,并通过免疫沉淀实验证明SKP2与OGG1之间存在相互作用。在氧化损伤环境下,SRA01/04细胞中SKP2蛋白表达出现先下降后逐渐升高的趋势,其中UVB照射10 min时SKP2表达下降最为显著。对照组、转染空载质粒组和转染SKP2过表达质粒组SRA01/04细胞中SKP2蛋白的相对表达量分别为1.040±0.007、0.920±0.008和1.330±0.020,与转染空载质粒组相比,转染SKP2过表达质粒组细胞中SKP2蛋白的表达显著上调(P<0.05)。空白对照组、UVB组、UVB+转染空载质粒组和UVB+转染SKP2过表达质粒组细胞中OGG1蛋白的相对表达量分别为1.05±0.01、5.05±0.16、5.20±0.07和3.83±0.10;与UVB+转染空载质粒组相比,UVB+转染SKP2过表达质粒组SRA01/04细胞中OGG1蛋白相对表达水平明显降低,且差异有统计学意义(P<0.05)。结论E3泛素连接酶SKP2能够促进OGG1发生泛素化降解,导致晶状体上皮细胞内部损伤性DNA的累积,从而导致ARC的发生发展。

原发性肝癌患者DNA损伤修复酶基因多态性分析

目的探讨DNA损伤修复酶基因多态性与原发性肝癌发生发展的关系。方法 PCR-RFLP法检测150例肝癌患者(肝癌组)和150例健康体检者(对照组)DNA损伤修复酶基因的表型,并进行比较。结果肝癌组XRCC1 Arg399Gln位点野生型的比率明显低于对照组(P<0.05);XRCC1(Arg194Trp、Arg280His)、hOGG1Ser326Cys位点多态性型别在两组中出现的频率相近(P>0.05);各基因位点不同表型者的尿8-羟基脱氧鸟苷(8-OHdG)水平相比,P均>0.05。结论 DNA修复酶基因多态性与肝癌的发生发展无明确的相关关系。

含有尿嘧啶DNA糖苷酶基因表达载体的构建

采用自行设计的带酶切位点的上下游引物，用PCR技术，从大肠杆菌ATCC23743的DNA中，获得了含有编码尿嘧啶DNA糖苷酶（UNG）基因的PCR产物，以该PCR产物构建了重组克隆质粒PGEM／UNG，DNA序列分析结果确证其中含有完整的UNG基因．利用该重组质粒，进一步构建了重组表达质料pBV／UNG．

评价替莫唑胺对脑胶质瘤治疗敏感性的新方法

背景与目的:替莫唑胺(temozolomide,TMZ)是治疗胶质母细胞瘤的唯一化疗药。O^6-甲基鸟嘌呤DNA甲基转移酶(O6-methylguanine-DNA methyltransferase,MGMT)基因启动子甲基化是评价TMZ敏感性的唯一指标。但通过检测MGMT的甲基化程度来评估TMZ的敏感性是不够的,因为目前MGMT检测只是定性检测,而且这种检测只能反映DNA损伤修复的一条通路,而另两条通路的修复情况却没有反映出来。方法:该研究一方面是应用高分辨率熔解曲线(high resolution melting,HRM),对MGMT的甲基化进行定量检测,同时应用实时荧光定量聚合酶链反应(real-time fluorescent quantitative polymerase chain reaction,RTFQPCR)来探讨另外两条修复通路蛋白N-甲基化嘌呤DNA糖基化酶(N-methylpurine DNA glycosylase,MPG)和人类烷烃羟化酶基因同系物2(alkane hydroxylase gene homolog 2,ALKBH2)的mRNA表达。将MPG和ALKBH2的表达分为高表达和低表达。结果:结合MGMT的甲基化(阳性)和非甲基化(阴性)程度,再把MPG和ALKBH2结合起来评估患者对TMZ的敏感性。三阳性(MGMT非甲基化,MPG阳性和ALKBH2阳性)为化疗抵抗,两阳性为不敏感,两阴性为次敏感,三阴性(MGMT甲基化,MPG阴性和ALKBH2阴性)为最敏感。结合8例胶质母细胞瘤患者的检测和生存期,结果与我们的判断结果相吻合,三阴性的患者生存时间最长,三阳性的患者的生存时间最短。结论:通过定量检测MGMT同时结合MPG和ALKBH2可以更精准地判断TMZ的敏感性。

Transforming growth factor-β and toll-like receptor-4 polymorphisms are not associated with fibrosis in haemochromatosis

AIM:To investigate the role of genetic polymorphisms in the progression of hepatic fibrosis in hereditary haemochromatosis.METHODS:A cohort of 245 well-characterised C282Y homozygous patients with haemochromatosis was studied,with all subjects having liver biopsy data and DNA available for testing.This study assessed the association of eight single nucleotide polymorphisms(SNPs)in a total of six genes including toll-like receptor 4(TLR4),transforming growth factor-beta(TGF-β),oxoguanine DNA glycosylase,monocyte chemoattractant protein 1,chemokine C-C motif receptor 2 and interleukin-10 with liver disease severity.Genotyping was performed using high resolution melt analysis and sequencing.The results were analysed in relation to the stage of hepatic fibrosis in multivariate analysis incorporating other cofactors including alcohol consumption and hepatic iron concentration.RESULTS:There were significant associations between the cofactors of male gender(P=0.0001),increasing age(P=0.006),alcohol consumption(P=0.0001),steatosis(P=0.03),hepatic iron concentration(P<0.0001)and the presence of hepatic fibrosis.Of the candidate gene polymorphisms studied,none showed a significant association with hepatic fibrosis in univariate or multivariate analysis incorporating cofactors.We also specifically studied patients with hepatic iron loading above threshold levels for cirrhosis and compared the genetic polymorphisms between those with no fibrosis vs cirrhosis however there was no significant effect from any of the candidate genes studied.Importantly,in this large,well characterised cohort of patients there was no association between SNPs for TGF-βor TLR4and the presence of fibrosis,cirrhosis or increasing fibrosis stage in multivariate analysis.CONCLUSION:In our large,well characterised group of haemochromatosis subjects we did not demonstrate any relationship between candidate gene polymorphisms and hepatic fibrosis or cirrhosis.