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DNA damage and repair of human skin keratinocytes concurrently exposed to pyrene derivatives and UVA light

机译:DNa损伤和人的皮肤的修复角质形成细胞同时暴露于芘衍生物和UVa光

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摘要

Polycyclic aromatic hydrocarbons (PAHs), a class of mutagenic environmental contaminants, insert toxicity through both metabolic activation and light irradiation. Pyrene, one of the most widely studied PAHs, along with its mono-substituted derivatives, 1-amino, 1-bromo, 1-hydroxy, and 1-nitropyrene, were chosen to study the effect of substituents on their phototoxicity, DNA damage and repair. Both alkaline Comet assay, which detects direct DNA damages, and Fpg endonuclease Comet assay, which detects oxidative DNA damages, were conducted at 0, 2, 4, 8, and 24 h of incubation of the cells in minimal growth medium after concomitant exposure to pyrene derivatives and UVA light. All these compounds are photocytotoxic and the phototoxicity is both incubation time and PAH dose dependent; whereas, those without light are not toxic. The LC50 obtained are in the range of 3.5 – 9.3 µM. Cellular DNA damages, both direct and oxidative, are observed immediately after the cells are treated with UVA light and the pyrene derivatives at a concentration of 1.0 µM. The amount of DNA damages (both direct and oxidative) increase from 0 to 4 h of incubation. After 4 hours, subsequent damage induction declines, and this is perceived to be mainly through DNA repair. After longer incubation of 8 h, the damaged cellular DNA start to be repaired, resulting in greatly reduced amount of DNA damages, and the DNA damage reaches the minimum at 24 h of incubation. 1-Amopyrene and 1-hydroxypyrene cause more DNA oxidative damages immediately after the exposure (0 h of incubation), and these damages are repaired within the same timeframe as the other tested compounds. The oxidative DNA damages caused by 1-bromopyrene are repaired starting at 2 h of incubation, earlier than the damages caused by all the other compounds.
机译:多环芳烃(PAHs)是一类致突变性环境污染物,可通过代谢活化和光照射而增加毒性。 studied是研究最广泛的PAH之一,连同其单取代衍生物1-氨基,1-溴,1-羟基和1-硝基py,用于研究取代基对其光毒性,DNA损伤和破坏的影响。修理。在暴露于最低限度的生长培养基中的细胞分别于0、2、4、8和24 h孵育后,进行检测直接DNA损伤的碱性Comet检测和检测氧化DNA损伤的Fpg内切核酸酶Comet检测。 derivatives衍生物和UVA光。所有这些化合物均具有光细胞毒性,并且光毒性既取决于孵育时间,又取决于PAH剂量。相反,没有光照的人没有毒性。获得的LC50在3.5 – 9.3 µM的范围内。在用浓度为1.0 µM的UVA光和the衍生物处理细胞后,立即观察到细胞DNA的直接和氧化损伤。 DNA损伤的数量(直接的和氧化的)从孵育的0小时增加到4小时。 4小时后,随后的损伤诱导下降,这被认为主要是通过DNA修复。长时间孵育8小时后,受损的细胞DNA开始被修复,从而大大减少了DNA损伤的数量,并且在孵育24小时后,DNA损伤达到了最小。暴露(孵育0小时)后,1-Amopyrene和1-hydroxypyrene造成更多的DNA氧化损伤,这些损伤在与其他测试化合物相同的时间内得到修复。在孵育2小时后,修复了由1-溴py引起的氧化DNA损伤,该损伤早于所有其他化合物引起的损伤。

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  • 年(卷),期 -1(2),3
  • 年度 -1
  • 页码 193–199
  • 总页数 14
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