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Dependence of the yields of AP sites and AP clusters produced in plasmid DNA on scavenging capacity and LET

机译:质粒DNA中产生的AP位点和AP簇的产量对清除能力和LET的依赖性

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摘要

An apurinic or apyrimidinic site (AP site) has known to be one of the typical DNA lesions induced by ionizing irradiation to cells. A clustered DNA damage site composed of AP sites (AP clusters) can be visualized as a double-strand break (DSB) by a treatment of DNA sample with endonuclease IV proteins as an enzymatic probe. AP clusters are efficiently induced in human cells by low LET γ- and X-irradiation [ ] with the similar yields with those for the clusters which contain pyrimidine or purine base lesions. However, there has been very little knowledge of the mechanistic aspects of the production of AP sites and AP clusters. Recently, we reported the dependence of the yields of AP sites and AP clusters, as well as base lesions, strand breaks and base lesion clusters induced by irradiation of carbon ions (LET: 13 and 60 keV/μm) obtained from HIMAC (NIRS, Chiba, Japan) on radical scavenging capacity in the DNA samples [ ].In the present study, we have performed theoretical calculation for the production of AP sites as well as those of strand breaks and base lesions by the carbon ion exposure (13 keV/μm). A Monte Carlo track structure simulation code for ion tracks, TRACION, was used for this work according to our previous study [ ]. As a DNA model molecule, simple linear DNA with 150 bp was applied for the calculation. Several scavenging capacities of the samples are tested to estimate the effect of indirect action of diffusible OH radicals in the damage induction in the experimental conditions.We assumed that the AP site formation pathway originates from a common intermediate of an OH radical adduct with that of single-strand breaks (SSBs) or base lesions (Scheme ). In order to reproduce the experimentally obtained yields of AP sites, we newly determined the branching ratio of induction of AP site to that of SSBs or base lesions to be 17:33 or 2:48, respectively, in the simulation. The calculated yields of AP site, as well as SSB, were well consistent with those for experimentally obtained (Fig. ). However, the calculated yields for AP clusters were one-fifth of those for experimental data. The yields for DSBs in lower scavenging capacities were also one-fifth of those for experimental ones in a lower scavenging capacity, thought they were well consistent with each other above a cell mimetic condition (>3 × 108 s). In order to bridge a gap between theoretical and experimental yields, we need a novel mechanism of damage-clustering such as dissociative low energy electron attachment or hole-migration onto a DNA molecule. Dependence of the yield of AP site or AP cluster (A) and prompt SSB or prompt DSB (B) on scavenging capacity in the sample. The experimental data below a scavenging capacity of 109 s are cited from [ ] and those at 1010 s in (B) are from [ ].
机译:已知嘌呤或嘧啶位点(AP位点)是通过电离辐射到细胞而诱导的典型DNA损伤之一。通过用核酸内切酶IV蛋白作为酶探针处理DNA样品,可以将由AP位点组成的簇状DNA损伤位点(AP簇)可视化为双链断裂(DSB)。通过低LETγ和X辐照[]可在人细胞中有效诱导AP簇,其收率与含有嘧啶或嘌呤碱基病变的簇相似。但是,对AP站点和AP群集的生产机制方面的知识很少。最近,我们报道了从HIMAC(NIRS,NIRS)获得的碳离子(LET:13和60 keV /μm)的辐照诱导的AP位点和AP簇的产量以及碱基病变,链断裂和碱基病变簇的产量的依赖性。 DNA样品中自由基清除能力的研究[]。在本研究中,我们已经进行了理论计算,计算了AP位点的产生,以及碳离子暴露(13 keV /微米)。根据我们先前的研究[],针对离子轨道的蒙特卡洛轨道结构仿真代码TRACION被用于这项工作。作为DNA模型分子,将150 bp的简单线性DNA用于计算。测试了样品的几种清除能力,以评估在实验条件下可扩散OH自由基对损伤诱导的间接作用的影响。我们假设AP位点形成途径起源于OH自由基加合物的共同中间体与单个-股断裂(SSBs)或基础病变(Scheme)。为了再现实验获得的AP位点的产量,我们在仿真中新确定了AP位点诱导与SSBs或基础病变的诱导分支比分别为17:33或2:48。 AP位点和SSB的计算产量与实验获得的产量完全一致(图)。但是,AP群集的计算出的产量是实验数据的五分之一。在较低的清除能力下,DSBs的产量也为在较低清除能力下的实验产品的五分之一,因为它们在模拟细胞的条件下(> 3×10 8 s)。为了弥合理论和实验产量之间的差距,我们需要一种新的损伤聚类机制,例如解离的低能电子附着或空穴迁移到DNA分子上。 <!-fig ft0-> <!-fig mode = article f1-> <!-caption a7->取决于AP站点或AP群集的产量(A)并提示SSB或提示DSB(B)清除样品中的容量。清除能力小于10 9 s的实验数据来自[],而(B)中10 10 s的实验数据来自[]。

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