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暴露于265 - 313纳米单色紫外波长和光复活光下的ICR 2A蛙细胞中姐妹染色单体交换的诱导。

Induction of sister-chromatid exchanges in ICR 2A frog cells exposed to 265-313 nm monochromatic ultraviolet wavelengths and photoreactivating light.

作者信息

Chao C C, Rosenstein R B, Rosenstein B S

出版信息

Mutat Res. 1985 May;149(3):443-50. doi: 10.1016/0027-5107(85)90162-9.

Abstract

Exposure of ICR 2A frog cells to 265 nm, 289 nm, 302 nm or 313 nm monochromatic ultraviolet (UV) wavelengths induced the formation of sister-chromatid exchanges (SCEs). However, treatment of cells with photoreactivating light (PRL) following the UV irradiations resulted in a lower level of SCEs compared with cells incubated in the dark. Hence, it can be concluded that pyrimidine dimers are the principal photoproducts responsible for the induction of SCEs in cells exposed to 265-313 nm UV due to the specificity of DNA photolyase for the light-dependent monomerization of dimers in DNA. It was also found that the maximum yield of induced SCEs in 313 nm-irradiated cells was only about 7 SCEs per cell whereas the plateau values for the shorter wavelengths were approximately 15-20 SCEs per cell. In addition, treatment of cells with 313 nm plus 265 nm light resulted in a lower level of SCEs than in cells exposed to 265 nm UV alone. These results can be interpreted in the context of a replication model for SCE, in which the high level of non-dimer damages produced in the DNA of 313 nm-irradiated cells inhibits the induction of SCEs by the pyrimidine dimers that are also produced by this wavelength.

摘要

将ICR 2A蛙细胞暴露于265纳米、289纳米、302纳米或313纳米的单色紫外线(UV)波长下会诱导姐妹染色单体交换(SCE)的形成。然而,紫外线照射后用光复活光(PRL)处理细胞,与在黑暗中孵育的细胞相比,SCE的水平较低。因此,可以得出结论,嘧啶二聚体是导致暴露于265 - 313纳米紫外线的细胞中SCE诱导的主要光产物,这是由于DNA光解酶对DNA中二聚体的光依赖性单体化具有特异性。还发现,在313纳米照射的细胞中,诱导SCE的最大产量仅约为每个细胞7个SCE,而较短波长的平稳值约为每个细胞15 - 20个SCE。此外,用313纳米加265纳米光处理细胞导致的SCE水平低于仅暴露于265纳米紫外线的细胞。这些结果可以在SCE的复制模型的背景下进行解释,在该模型中,313纳米照射的细胞DNA中产生的高水平非二聚体损伤会抑制该波长也产生的嘧啶二聚体对SCE的诱导。

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