Induction and Rejoining of DNA Double-Strand Breaks in Normal Human Skin Fibroblasts after Exposure to Radiation of Different Linear Energy Transfer: Possible Roles of Track Structure and Chromatin Organization

Höglund, E. and Stenerlöw, B. Induction and Rejoining of DNA Double-Strand Breaks in Normal Human Skin Fibroblasts after Exposure to Radiation of Different Linear Energy Transfer: Possible Roles of Track Structure and Chromatin Organization. Radiat. Res. 155, 816–823 (2001). DNA double-strand breaks...

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Veröffentlicht in:Radiation research 2001-06, Vol.155 (6), p.818-825
Hauptverfasser: Hoeglund, Erik, Stenerloew, Bo
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Sprache:eng
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Zusammenfassung:Höglund, E. and Stenerlöw, B. Induction and Rejoining of DNA Double-Strand Breaks in Normal Human Skin Fibroblasts after Exposure to Radiation of Different Linear Energy Transfer: Possible Roles of Track Structure and Chromatin Organization. Radiat. Res. 155, 816–823 (2001). DNA double-strand breaks are nonrandomly induced by high-LET radiation. Differences in the induction and rejoining of DSBs after irradiation with ions having different LET were detected by fragment analysis. The data obtained indicate that the track structure of the traversing particle and its interaction with the different chromatin structures of the cellular DNA influence the yield as well as the distribution of the induced damage. The induction and rejoining of clustered DSBs induced by the same nitrogen ion fluence at LETs of 80–225 keV/μm were investigated by a detailed analysis of the DNA fragmentation patterns in normal human fibroblasts. The DSBs in the cells were allowed to rejoin during incubations for 0–20 h. Two separate pulsed-field gel electrophoresis protocols were used, optimized for separation of fragments in the size ranges 1–6 Mbp and 5 kbp–1.5 Mbp. A strong influence of LET on the level of DSB induction was evident. The DSB yield increased from 4.5 ± 0.2 to 10.0 ± 0.3 DSBs per particle traversal through the cell nucleus when LET increased from 80 to 225 keV/μm. Further, the size distribution of the DNA fragments showed a significant dependence on radiation quality, with an excess of fragments at 50–200 kbp and around 1 Mbp. Differences in repair kinetics were also evident, with slower rejoining for increasing LET, and the initial nonrandom fragment distributions were still present after 1 h of repair.
ISSN:0033-7587
1938-5404
DOI:10.1667/0033-7587(2001)155[0818:IARODD]2.0.CO;2