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Is the Comet Assay a Sensitive Procedure for Detecting Genotoxicity?

机译:彗星试验是检测基因毒性的灵敏方法吗?

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摘要

Although the Comet assay, a procedure for quantitating DNA damage in mammalian cells, is considered sensitive, it has never been ascertained that its sensitivity is higher than the sensitivity of other genotoxicity assays in mammalian cells. To determine whether the power of the Comet assay to detect a low level of genotoxic potential is superior to those of other genotoxicity assays in mammalian cells, we compared the results of Comet assay with those of micronucleus test (MN test). WTK1 human lymphoblastoid cells were exposed to methyl nitrosourea (MNU), ethyl nitrosourea (ENU), methyl methanesulfonate (MMS), ethyl methanesulfonate (EMS), bleomycin (BLM), or UVC. In Comet assay, cells were exposed to each mutagen with (Comet assay/araC) and without (Comet assay) DNA repair inhibitors (araC and hydroxyurea). Furthermore, acellular Comet assay (acellular assay) was performed to determine how single-strand breaks (SSBs) as the initial damage contributes to DNA migration and/or to micronucleus formation. The lowest genotoxic dose (LGD), which is defined as the lowest dose at which each mutagen causes a positive response on each genotoxicity assay, was used to compare the power of the Comet assay to detect a low level of genotoxic potential and that of MN test; that is, a low LGD indicates a high power. Results are summarized as follows: (1) for all mutagens studied, LGDs were MN test ≦ Comet assay; (2) except for BLM, LGDs were Comet assay/araC ≦ MN test; (3) except for UVC and MNU, LGDs were acellular assay ≦ Comet assay/araC ≦ MN test ≦ Comet assay. The following is suggested by the present findings: (1) LGD in the Comet assay is higher than that in MN test, which suggests that the power of the MN test to detect a low level of genotoxic potential is superior to that of the Comet assay; (2) for the studied mutagens, all assays were able to detect all mutagens correctly, which suggests that the sensitivity of the Comet assay and that of the MN test were exactly identical; (3) the power of the Comet assay to detect a low level of genotoxic potential can be elevated to a level higher than that of MN test by using DNA resynthesis inhibitors, such as araC and HU.
机译:尽管彗星试验是一种定量分析哺乳动物细胞中DNA损伤的方法,但被认为是敏感的,但从未确定其敏感性高于哺乳动物细胞中其他遗传毒性试验的敏感性。为了确定彗星试验在哺乳动物细胞中检测低水平遗传毒性潜力的能力是否优于其他遗传毒性试验,我们将彗星试验的结果与微核试验(MN试验)的结果进行了比较。将WTK1人类淋巴母细胞暴露于亚硝基甲基(MNU),亚硝基乙基(ENU),甲磺酸甲酯(MMS),甲磺酸乙酯(EMS),博来霉素(BLM)或UVC。在彗星试验中,将细胞暴露于每种诱变剂中(使用Comet分析/ araC)和不使用(Comet分析)DNA修复抑制剂(araC和羟基脲)。此外,进行了脱细胞彗星试验(脱细胞试验),以确定初始损伤时单链断裂(SSB)如何促进DNA迁移和/或微核形成。最低遗传毒性剂量(LGD)定义为每种诱变剂在每次遗传毒性分析中引起阳性反应的最低剂量,用于比较Comet分析检测低水平遗传毒性潜力和MN的能力测试;也就是说,低LGD表示高功率。结果总结如下:(1)对于所有研究的诱变剂,LGD均进行MN检验≦彗星试验; (2)除BLM外,LGD均为彗星试验/ araC≦MN试验; (3)除UVC和MNU外,LGDs分别为脱细胞分析≤Comet分析/ araC≤MN test≤Comet分析。本研究结果表明:(1)彗星试验中的LGD高于MN试验中的LGD,这表明MN试验检测低水平遗传毒性潜力的能力优于彗星试验。 ; (2)对于所研究的诱变剂,所有测定法都能正确检测所有诱变剂,这表明彗星测定法和MN试验的灵敏度完全相同; (3)通过使用araC和HU等DNA再合成抑制剂,可以将Comet分析检测低水平遗传毒性潜力的能力提高到比MN试验更高的水平。

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