Nicotine interacts with DNA lesions induced by alpha radiation which may contribute to erroneous repair in human lung epithelial cells

Nadia Boroumand
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Abstract

Purpose: Epidemiological studies show that radon and cigarette smoke interact in inducing lung cancer, but the contribution of nicotine in response to alpha radiation emitted by radon is not well understood. Materials and methods: Bronchial epithelial BEAS 2B cells were either pre-treated with 2 uM nicotine during 16 h, exposed to radiation, or the combination. DNA damage, cellular and chromosomal alterations, oxidative stress as well as inflammatory responses were assessed to investigate the role of nicotine in modulating responses. Results: Less γH2AX foci were detected at 1 h after alpha radiation exposure (1 2 Gy) in the combination group versus alpha radiation alone, whereas nicotine alone had no effect. Comet assay showed less DNA breaks already just after combined exposure, supported by reduced p-ATM, p DNA PK, p p53 and RAD51 at 1 h, compared to alpha radiation alone. Yet the frequency of translocations was higher in the combination group at 27 h after irradiation. Although nicotine did not alter G2 arrest at 24 h, it assisted in cell cycle progression at 48 h post radiation. A slightly faster recovery was indicated in the combination group based on cell viability kinetics and viable cell counts, and significantly using colony formation assay. Pan-histone acetyl transferase inhibition using PU139 blocked the reduction in p p53 and γH2AX activation, suggesting a role for nicotine-induced histone acetylation in enabling rapid DNA repair. Nicotine had a modest effect on reactive oxygen species induction but tended to increase alpha particle induced pro inflammatory IL 6 and IL 1β (4 Gy). Interestingly, nicotine did not alter gamma radiation induced γH2AX foci. Conclusions: This study provides evidence that nicotine modulates alpha radiation response by causing a faster but more error prone repair, as well as rapid recovery, which may allow expansion of cells with genomic instabilities. These results hold implications for estimating radiation risk among nicotine users.
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尼古丁与阿尔法辐射诱导的 DNA 损伤相互作用,可能导致人类肺上皮细胞的错误修复
目的:流行病学研究表明,氡和香烟烟雾在诱发肺癌方面具有相互作用,但尼古丁对氡发出的α辐射的影响尚不十分清楚。材料和方法:将支气管上皮 BEAS 2B 细胞用 2 uM 尼古丁预处理 16 小时、暴露于辐射或两者结合。评估DNA损伤、细胞和染色体改变、氧化应激以及炎症反应,以研究尼古丁在调节反应中的作用。结果显示α射线照射(1 2 Gy)1小时后,联合组检测到的γH2AX病灶少于单独照射组,而单独使用尼古丁则没有影响。彗星试验显示,与单独使用α射线相比,联合照射后 1 小时,p-ATM、p DNA PK、p p53 和 RAD51 减少,DNA 断裂减少。然而,在照射后 27 小时,联合组的易位频率更高。虽然尼古丁不会改变辐射后24小时的G2停滞,但却有助于辐射后48小时的细胞周期进展。根据细胞存活动力学和存活细胞计数以及菌落形成检测,联合组的恢复速度稍快。使用 PU139 抑制泛组蛋白乙酰转移酶可以阻止 p p53 和 γH2AX 活化的减少,这表明尼古丁诱导的组蛋白乙酰化在快速修复 DNA 方面发挥了作用。尼古丁对活性氧的诱导作用不大,但往往会增加α粒子诱导的促炎 IL 6 和 IL 1β(4 Gy)。有趣的是,尼古丁并未改变伽马射线诱导的γH2AX病灶:本研究提供的证据表明,尼古丁可通过导致更快但更容易出错的修复以及快速恢复来调节α辐射反应,从而使基因组不稳定的细胞得以扩增。这些结果对估计尼古丁使用者的辐射风险具有一定的意义。
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