DNA Double-Strand Breaks,Potential Targets for HBV Integration

Hepatitis B virus(HBV)-induced hepatocellular carcinoma(HCC) is one of the most fre-quently occurring cancers.Hepadnaviral DNA integrations are considered to be essential agents which can promote the process of the hepatocarcinogenesis.More and more researches were designed to find the relationship of the two.In this study,we investigated whether HBV DNA integration occurred at sites of DNA double-strand breaks(DSBs),one of the most detrimental DNA damage.An 18-bp I-SceI homing endonuclease recognition site was introduced into the DNA of HepG2 cell line by stable DNA transfection,then cells were incubated in patients’ serum with high HBV DNA copies and at the same time,DSBs were induced by transient expression of I-SceI after transfection of an I-SceI expression vector.By using nest PCR,the viral DNA was detected at the sites of the break.It appeared that integra-tion occurred between part of HBV x gene and the I-SceI induced breaks.The results suggested that DSBs,as the DNA damages,may serve as potential targets for hepadnaviral DNA insertion and the integrants would lead to widespread host genome changes necessarily.It provided a new site to investi-gate the integration.

Comparison of DNA double-strand breaks induced by ^(16)O^(8+) in deproteinized DNA and intact cells

The yield of DNA double-strand breaks (DSBs) is sure to be influenced by theenvironment around DNA molecule. Inverse pulsed-field gel electrophoresis (PIGE) has beenapplied to compare the sensitivity of B16 cells and their DNA in DSBs induced by 75 MeV/u16O8+ beam. Results show that the percentages of DNA released from the plug(PR) in bothkinds of tile samples increase with the dose and approach a similar quasi-threshold of about81%. A simple new equation was presented to calculate the break level of DNA molecules.Within a certain dose, the relationship between the break level and the dose is linear. Theyield of DSBs in deproteinized DNA was 1.11 DSBs/100 Mbp/Gy, while that in intact cells was0.60DSBs/100Mbp/Gy. It is testified that deproteinized DNA is more sensitive to oxygen ionsirradiation than intact cells.

Exposure to Long Magnetic Resonance Imaging Thermometry Does Not Cause Significant DNA Double-Strand Breaks on CF-1 Mice

The purpose of the study was to investigate if the high gradient strength and slew rate used for long MRI-thermometry monitoring could cause DNA double-stranded breaks (DSBs). To this end, an enzyme-linked immunosorbent assay (ELISA) was used to quantify γH2AX, a molecular marker for DSBs, in the blood of mice after a 6-hour exposure to magnetic resonance imaging (MRI). Fourteen CF-1 female mice were separated into 4 experimental groups: Untreated negative control, MRI-treated, MRI-Control, and exposed to ionizing radiation positive control. Untreated negative control was used as a baseline for ELISA to quantify γH2AX. MRI-treated consisted of a 6-hour continuous magnetic resonance imaging (MRI) echo planar imaging (EPI) sequence with a slew rate of 192 mT/m/s constituting a significantly longer imaging time than routine clinical imaging. MRI-control mice were maintained under the same conditions outside the MRI scanner for 6-hours. Mice in the irradiation group served as a positive control of DSBs and were exposed to either 2 Gy, 5 Gy or 10 Gy of ionizing radiation. DSBs in the blood lymphocytes from the treatment groups were analyzed using the γH2AX ELISA and compared. Total protein concentration in lysates was determined for each blood sample and averaged 1 ± 0.35 mg/mL. Irradiated positive controls were used to test radiation dose-dependency of the γH2AX ELISA assay where a linear dependency on radiation exposure was observed (r2 = 0.93) between untreated and irradiated samples. Mean and standard error mean of γH2AX formation were calculated and compared between each treatment group. Repeated measures 1-way ANOVA showed statistically significant differences between the means of irradiated controls and both the MRI-control and MRI-treated groups. There was no statistically significant difference between the MRI-treated samples and the MRI-control groups. Our results show that long MRI exposure at a high slew rate did not cause increased levels of γH2AX when compared to control mice, suggesting that no increase in DSBs was caused by the long MR thermometry imaging session. The novelty of this work contradicts other studies that have suggested MRI may cause DSBs;this work suggests an alternative cause of DNA damage.

The role of NBS1 in DNA double strand break repair, telomere stability, and cell cycle checkpoint control

The genomes of eukaryotic cells are under continuous assault by environmental agents and endogenous metabolic byproducts. Damage induced in DNA usually leads to a cascade of cellular events, the DNA damage response. Failure of the DNA damage response can lead to development of malignancy by reducing the efficiency and fidelity of DNA repair. The NBS1 protein is a component of the MRE11/RAD50/NBS 1 complex （MRN） that plays a critical role in the cellular response to DNA damage and the maintenance of chromosomal integrity. Mutations in the NBS1 gene are responsible for Nijmegen breakage syndrome （NBS）, a hereditary disorder that imparts an increased predisposition to development of malignancy. The phenotypic characteristics of cells isolated from NBS patients point to a deficiency in the repair of DNA double strand breaks. Here, we review the current knowledge of the role of NBS1 in the DNA damage response. Emphasis is placed on the role of NBS1 in the DNA double strand repair, modulation of the DNA damage sensing and signaling, cell cycle checkpoint control and maintenance oftelomere stability.

Maternal gene Ooep may participate in homologous recombination-mediated DNA double-strand break repair in mouse oocytes

DNA damage in oocytes can cause infertility and birth defects. DNA double-strand breaks （DSBs） are highly deleterious and can substantially impair genome integrity. Homologous recombination （HR）-mediated DNA DSB repair plays dominant roles in safeguarding oocyte quantity and quality. However, little is known regarding the key players of the HR repair pathway in oocytes. Here, we identified oocyte-specific gene Ooep as a novel key component of the HR repair pathway in mouse oocytes. OOEP was required for efficient ataxia telangiectasia mutated （ATM） kinase activation and Rad51 recombinase （RAD51） focal accumulation at DNA DSBs. Ooep null oocytes were defective in DNA DSB repair and prone to apoptosis upon exogenous DNA damage insults. Moreover, Ooep null oocytes exhibited delayed meiotic maturation. Therefore, OOEP played roles in preserving oocyte quantity and quality by maintaining genome stability. Ooep expression decreased with the advance of maternal age, suggesting its involvement in maternal aging.

DETECTION OF STRAND BREAKS OF DNA IN HUMAN EARLY CHORIONIC VILLUS CELLS INDUCED BY DIAGNOSTIC ULTRASOUND USING ^(32)P-LABELED ALU HYBRIDIZATION

Objective To explore if strand breaks of DNA in human early chorionic villus cells in uterus were induced by diagnostic ultrasound and to evaluate the method used for detection of single-stranded breaks and double-stranded breaks in human DNA. Methods 60 normal pregnant women aged 20-30, who underwent artificial abortion during 6-8 weeks of gestation, were randomly divided into 2 experimental groups: All 30 cases were exposed to diagnostic ultrasound in uterus for 10 minutes, and 24 hours later chorionic villi were extracted; the other 30 cases were taken as the control group. Single-stranded DNA and double-stranded DNA in villus cells in all cases were isolated by the alkaline unwinding combined with hydroxylapatite chromatography, and were quantitatively detected using 32 P-labeled Alu probe for dot-blotting hybridization. Results There was no significant difference in quantity and percentage in single-stranded DNA and double-stranded DNA between 2 groups (P>0.05). 32 P-Alu probe could only hybridize with human DNA, and could detect DNA isolated from as few as 2.5×10 3 chorionic villus cells and 0.45ng DNA in human leukocytes. Conclusion The results suggested that there were no DNA strand damages in human chorionic villus cells when the uterus was exposed to diagnostic ultrasound for 10 minutes. The method,^(32)P-Alu probe for dot-blotting hybridization, was even more specific, sensitive and accurate than conventional approaches.

DNA聚合酶θ:易错的多功能DNA末端修复分子

DNA聚合酶θ(DNA polymerase theta,Polθ)是一种广泛存在于动植物中的DNA修复酶。它在选择性末端连接(alternative end-joining,Alt-EJ)途径中发挥着关键作用,常参与DNA双链断裂(DNA double-strand breaks,DSB)损伤修复。在正常生理状态下,Polθ主要调控基因组稳定性。然而,在恶性肿瘤发生时,Polθ表现出异常高表达水平,并参与调控肿瘤细胞的恶性转变过程。研究表明,抑制Polθ活性可导致同源重组(homologous recombination,HR)缺陷的肿瘤细胞发生合成致死(synthetic lethality,SL)。因此,已经开发出多种针对Polθ的小分子抑制剂,可与其他化疗药物联合使用以抑制恶性肿瘤的发展。此外,敲除或抑制Polθ活性还能增加HR修复效率,从而提高外源基因靶向整合效果。本文综述了Polθ及其介导的Alt-EJ修复机制在生物学功能方面的最新研究进展,为靶向Polθ在肿瘤治疗和基因编辑方面的应用提供理论基础。

川芎嗪通过RAD52调控乳腺癌细胞DNA损伤修复

目的:探究TMP对乳腺癌BT474细胞增殖、细胞周期及其调控蛋白表达与DNA双链断裂修复通路的相关性。方法:CCK8法测定TMP对乳腺癌BT474细胞的增殖抑制情况;流式细胞术测定TMP对细胞周期的影响;单细胞凝胶电泳测定分析TMP对损伤后细胞DSBs累积情况的影响;Isce-I内切酶系统检测TMP对修复通路活性的影响;Western blotting检测DSBs修复通路相关染色体结合蛋白表达水平变化。结果:TMP通过使细胞阻滞在G_(1)期呈浓度依赖性抑制BT474细胞增殖,显著减少体内由Zeocin导致的细胞拖尾DNA含量(P<0.05);TMP显著增加BT474细胞对RAD52、ERCC1、XRCC4以及DNA LigⅣ蛋白募集,减少对KU80蛋白募集,促进了SSA以及NHEJ通路修复活性(P<0.05)。结论:TMP通过阻滞BT474细胞停留在G_(1)期使其发挥增殖抑制作用的机制之一;TMP通过增强损伤缺口对各个通路的关键染色体结合蛋白募集,促进SSA与NHEJ修复通路活性从而减少DNA损伤。

重离子辐照诱导DNA双链断裂的剂量率效应

利用不同剂量率的 5 0MeV/u12C6+ 辐照B16黑色素瘤细胞的脱蛋白DNA ,采用脉冲场凝胶电泳技术对DNA双链断裂 (DSB)的诱导和片段的分布进行了研究。结果发现 ,在剂量率分别为3Gy/min和 30Gy/min的情况下 ,DNA片段释放百分比 (PR)都随着剂量的增加而增加 ,并在超过一定剂量之后趋于相似的准阈值 ;3Gy/min辐照诱导DSB的产额为 0 .4 0DSBs/ (10 0Mbp .Gy) ,30Gy/min辐照诱导的DSB产额准确值无法得到 ;30Gy/min辐照诱导DSB的截面为 2 .14μm2 ,是 3Gy/min的 3.1倍。所有结果都表明剂量率越高 ,诱导DSB越有效。另外 ,3Gy/min辐照诱导DSB片段在 -86 0kbp处有一个片段峰 ,而 30Gy/min没有 ,说明剂量率可以影响DSB片段的分布。

γ射线诱导的肝癌细胞DNA双链断裂

为了揭示辐射生物学效应的机理，用倒转脉冲场凝胶电泳（ＰＩＧＥ）研究了γ射线辐照肝癌ＳＭＭＣ—７７２１细胞诱导的ＤＮＡ双链断裂（ＤＳＢ）及其修复２４、４８ｈ后的产额和片段的分布情况。结果表明：修复０ｈ和２４ｈ的样品，ＤＮＡ片段释放百分比（ＰＲ）随着剂量的增加而增加；诱导的ＤＳＢ片段主要是 １Ｍｂｐ— ２Ｍｂｐ的大片段； ＤＳＢ产额分别为 ０．３８ＤＳＢｓ／１００Ｍｂｐ· Ｇｙ和０．０６ＤＳＢｓ／１００Ｍｂｐ·Ｇｙ，即２４ｈ内，约８４％的ＤＳＢ发生了重接；修复４８ｈ后残余的ＤＳＢ片段与剂量无关，且与对照细胞的ＤＳＢ片段含量相近。可见，γ射线诱导的ＤＳＢ容易发生修复；未修复的ＤＳＢ将导致细胞的增殖死亡。

DNA-PKcs在鼻咽癌组织中的表达及其临床意义

背景与目的:DNA双链断裂(DNA double-strand break,DSB)是射线杀灭肿瘤细胞的主要机制,而同源重组(homologous recombination,HR)和非同源性末端连接(DNA nonhomologous end-joining,NHEJ)是DSB的两条重要修复途径。DNA-PK催化亚单位(catalytic subunit of DNA-dependent protein kinase,DNA-PKcs)是NHEJ途径的主要修复蛋白之一,在DSB中发挥着重要作用。本研究旨在通过检测鼻咽癌组织中DNA-PKcs的表达情况,探讨其与鼻咽癌临床病理特征及预后的关系。方法:采用免疫组化SP法检测223例鼻咽癌患者组织中DNA-PKcs的表达,并结合患者的临床及预后资料进行分析。结果:223例鼻咽癌患者中,DNA-PKcs的过表达率为36.8%。卡方检验显示,DNA-PKcs表达强弱与患者的性别、年龄、病理分型及N分期的相关性均无统计学意义(P>0.05),与TNM分期、T分期、M分期均有关(P<0.05)。单因素生存分析显示,DNA-PKcs过表达患者5年总生存率低于低表达患者(54.6%vs.79.4%),差异有统计学意义(P<0.05)。多因素Cox回归模型分析显示T、N、M分期及DNA-PKcs表达水平是影响鼻咽癌患者预后的独立因素(P<0.05)。结论:DNA-PKcs在大部分鼻咽癌组织中均有表达,DNA-PKcs的表达水平与鼻咽癌患者预后相关,对患者的预后判断有一定的指导意义。

乳腺癌易感基因1在DNA损伤修复中作用的研究进展

乳腺癌易感基因1(BRCA1)基因突变与乳腺癌的发生密切相关。目前研究表明,BRCA1作为调节者参与了DNA损伤修复过程。DNA损伤的最严重的形式是双链断裂,BRCA1通过调控同源重组(HR)在修复双链断裂中发挥关键作用。本文从BRCA1主要功能区与HR的关系、主要功能区基因突变对修复双链断裂的影响、BRCA1与BRCA2,Rad51和CtIP复合物等蛋白之间的相互作用和蛋白的磷酸化等方面,对BRCA1调控HR的分子机制、BRCA1介导的修复机制缺失在合成致死性中的作用、及BRCA1缺失后细胞对不同DNA损伤制剂敏感性发生的变化等内容进行了系统的综述。

电离辐射诱导的DNA双链断裂

利用γ射线和不同LET的碳离子辐照小鼠B16黑色素瘤细胞、Hela细胞、V79中国仓鼠肺细胞和人肝癌SMMC -7721细胞的DNA ,采用脉冲场凝胶电泳结合荧光扫描技术研究了DNA双链断裂(DSB)片段的分布。结果发现DSB片段是非随机分布的 ,而且这种分布与DNA序列有关。原因可能在于沉积的能量直接或间接沿DNA链迁移 ,链上相对较弱的化学键优先产生反应 ,并最终导致链的断裂 ,从而引起断裂的不均匀分布。

不育患者精子DNA链损伤类型的研究及临床意义

目的:观察精子DNA单、双链损伤(SSB、DSB)在男性不育中的特征,探讨DSB与男性不育的关系,为男性不育的诊疗提供新的观察指标与思路。方法:选择男性不育患者60例以及同期因女方因素不孕前来检查的生育力评估正常的健康男性30例作为对照组,分析两组精子DNA损伤及精液主要参数的差异。精子浓度及活力采用计算机辅助精子分析系统,精子存活率分析采用低渗膨胀试验,精子形态采用Diff-Quik染色法,精子DNA损伤采用双尾彗星实验。结果:双尾彗星实验检测精子DNA完整性共有9种彗星模型。不育患者精子DNA损伤指数(DFI)为(33.8±13.1)%,单链损伤指数(SSB-DFI)为(19.2±11.4)%、SSB占所有损伤精子的比率(SSB-DFI/DFI)为(56.8±32.4)%,双链损伤指数(DSB-DFI)为(23.9±13.4)%、DSB占所有损伤精子的比率(DSB-DFI/DFI)为(70.8±19.5)%;与对照组比较[分别为(16.3±7.9)%、(14.9±7.6)%、(91.4±27.8)%、(6.1±2.7)%、(37.4±11.3)%)],SSB-DFI无显著性差异(P>0.05),DSB-DFI、DFI和DSB-DFI/DFI显著高于对照组(P均<0.01),SSB-DFI/DFI显著降低于对照组(P<0.01)。绘制ROC曲线,DSB-DFI/DFI、DSB-DFI及DFI诊断男性不育最佳截断值分别为39.5%、15.85%和18.65%,ROCAUC、敏感度和特异性分别为(0.969,98.3%,90.0%)、(0.912,86.7%,80.0%)、(0.861,90.0%,70.0%)。不育组精子SSB-DFI及SSB-DFI/DFI与精液常规参数均无相关关系(P均>0.05),DFI与前向运动精子百分率、精子存活率及正常形态精子百分率呈负相关(P<0.05或P<0.01),与精子浓度无相关关系(P>0.05),精子DSB-DFI及DSB-DFI/DFI与精子浓度、精子存活率、前向运动精子百分率及正常形态精子百分率均呈负相关(P<0.05或P<0.01)。结论:影响男性不育的DAN损伤因素可能是DSB,而与SSB相关性不大,精子DNA链的损伤类型对男性生殖能力的评估有较大的参考价值。

单细胞凝胶电泳检测外照射诱导DNA单链断裂和双链断裂

分别应用中性单细胞凝胶电泳、碱性单细胞凝胶电泳技术检测了不同剂量γ射线外照射对小鼠外周血淋巴细胞DNA的损伤。结果表明 ,γ射线外照射对小鼠外周血淋巴细胞DNA具有明显的损伤作用 ,彗星细胞百分率显著增加 ,DNA电泳迁移 。

恒场电泳检测DNA双链断裂及其应用

应用普通恒场琼脂糖凝胶电泳检测受γ射线照射后小鼠胸腺细胞ＤＮＡ双链断裂（ｄｓｂ）。在一定条件下，该法可以获得与脉冲凝胶电泳相似的结果。用此法观察了离体照射小鼠胸腺细胞ＤＮＡｄｓｂ修复作用，发现该法可以检测到ＤＮＡ“梯状”带，可做为一种研究细胞凋亡的新方法。

电离辐射诱发小鼠脾细胞DNA链断裂及修复

目的通过观察γ射线照射后IRM-2辐射抗性小鼠DNA链的断裂及修复,探讨IRM-2小鼠辐射抗性产生的可能机理。方法采用脉冲场凝胶电泳法,测定不同剂量γ射线诱发IRM-2小鼠及其亲本ICR/JCL和615小鼠脾细胞DNA单、双链断裂及照射后不同时间DNA链断裂的修复动力学。结果对照组IRM-2小鼠本底DNA损伤较低,即ssb和dsb的数目低于未照射的亲本ICR和615小鼠(P<0.01)。不同剂量(1、2、4和8Gy)照射后,IRM-2小鼠ssb和dsb的数量均明显低于经相同剂量照射的亲本ICR和615小鼠(P<0.05和P<0.01)。在较低剂量2Gy时,IRM-2小鼠与亲本小鼠相比,dsb和ssb修复无统计学差异;当分别接受4、8Gy大剂量照射后,IRM-2小鼠表现出较高的修复效率,即IRM-2小鼠0.5h和1hdsb、ssb修复速率比亲本小鼠快(P<0.05和P<0.01),而且修复后剩余的损伤远低于亲本小鼠。结论电离辐射后IRM-2小鼠DNA链断裂量较低,DNA链断裂的修复速率比亲本小鼠快,因此能及时快速地抵抗辐射造成的损伤,具有较强的辐射抗性。

氧氟沙星对锦鲤抗氧化系统和DNA损伤的影响

由于抗生素对人体健康和生态环境潜在的威胁,其大量使用已引起人们广泛关注。该研究通过毒性暴露试验,研究了氟喹诺酮类抗生素氧氟沙星(OFLX)对锦鲤抗氧化酶活性和DNA损伤的影响。结果表明,随着暴露浓度和时间的增加,OFLX对锦鲤鱼肝SOD活性、MDA和GST含量呈现显著的诱导效应。当OFLX浓度200 mg/L,暴露13 d时,锦鲤肝脏各项抗氧化酶活性指标均出现显著降低,表明OFLX对锦鲤的抗氧化系统的累积毒性超出了鱼体的自身调节能力,导致鱼体的抗氧化系统的损伤。鱼鳃组蛋白H2AX(γ-H2AX)磷酸化结果表明,OFLX可造成鱼体DNA损伤,诱导鱼鳃γ-H2AX产生和簇集,且呈现明显的剂量-效应关系。OFLX浓度200 mg/L,暴露4 d时鱼鳃γ-H2AX浓度达到最大值(110.49 ng/L)。随着暴露时间继续增加,各浓度组γ-H2AX含量均有所下降,表明OFLX可能导致造成DNA双链的断裂,导致γ-H2AX浓度下降。该结果为评估OFLX对锦鲤的抗氧化系统和DNA毒性影响提供了较为可靠的依据。

X射线辐照诱导人神经胶质瘤细胞DNA双链损伤研究

采用免疫荧光染色法检测X射线诱导M059K细胞磷酸化组蛋白H2AX(γH2AX)和磷酸化的毛细血管扩张性共济失调症突变基因(pATM)焦点的形成;流式细胞仪分析M059K细胞γH2AX和pATM表达的周期依赖性。免疫荧光染色检测结果显示,γH2AX和pATM焦点阳性细胞分别以照射后0.5、4 h表达最高,照射后24h,高剂量组焦点阳性细胞达100%。流式细胞仪分析结果显示,γH2AX和pATM的表达具有细胞周期依赖性。照射后0.5、4 h,γH2AX和pATM在细胞各期的表达均明显增加,并以G0/G1期为著;照射后24 h,γH2AX和pATM在G0/G1和S期表达降低,而G2/M期细胞表达明显增加。细胞呈现明显的G2/M期阻滞。结果提示,γH2AX和ATM信号通路参与X射线诱导的M059K细胞DNA双链断裂。

重离子诱导的质粒DNA双链断裂分布研究

利用能量为7.2MeV/u氖离子束辐照体外质粒DNA:pUC18,采用恒场凝胶电泳结合多功能荧光成像系统研究了pUC18双链断裂片段的分布。证实了双链断裂片段分布的非随机性,结果还发现DNA断裂后片段的交联现象,而且交联片段的分布也是非随机的。