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Ultraviolet light induces double-strand breaks in DNA of cultured human P3 cells as measured by neutral filter elution.

作者信息

Peak J G, Peak M J

机构信息

Molecular Photobiology Group, Argonne National Laboratory, IL 60439-4833.

出版信息

Photochem Photobiol. 1990 Aug;52(2):387-93. doi: 10.1111/j.1751-1097.1990.tb04194.x.

DOI:10.1111/j.1751-1097.1990.tb04194.x
PMID:2217550
Abstract

Neutral filter elution at pH 7.2 and 9.6 was used to measure the induction of DNA lesions in human P3 teratocarcinoma cells by monochromatic 254-, 270-, 313-, 334-, 365-, and 405-nm radiation and by 60 gamma rays. In this assay DNA double-strand breaks (dsb) increase the rate of elution of DNA from cell lysates on a filter. Yields of dsb as measured by this procedure were determined by using a calibration of the assay that correlates elution parameters with number of dsb caused by disintegration of 125I incorporated into the DNA. Analysis of fluence responses obtained by using the calibrated assay indicated that the number of dsb induced per dalton of DNA as measured by this assay is proportional to the square of the fluence at all the energies of radiation studied, implying that the induction of these lesions may be a two-hit event. Analysis of the relative efficiencies for the induction of dsb by ultraviolet radiation, corrected for quantum efficiency, revealed a spectrum that coincided closely with that for the induction of single-strand breaks (ssb) in the same cells, having a close fit with the spectrum of nucleic acid in the UVC and UVB region below 313 nm, and a shoulder in the UVA region. It was calculated, however, that there may be too few ssb for dsb to result from randomly distributed closely opposed ssb.

摘要

相似文献

1
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Photochem Photobiol. 1990 Aug;52(2):387-93. doi: 10.1111/j.1751-1097.1990.tb04194.x.
2
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Measurement of double-strand breaks in Chinese hamster cell DNA by neutral filter elution: calibration by 125I decay.通过中性滤膜洗脱法测量中国仓鼠细胞DNA中的双链断裂:用¹²⁵I衰变进行校准
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