Analysis of nucleotide excision repair by detection of single-stranded DNA transients

doi:10.1093/carcin/22.11.1789

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Carcinogenesis, Vol. 22, No. 11, 1789-1796, November 2001
© 2001 Oxford University Press

CANCER BIOLOGY

Analysis of nucleotide excision repair by detection of single-stranded DNA transients

Carlos P. Rubbi^,1 and Jo Milner

YCR P53 Research Group, Department of Biology, University of York, York YO10 5DD, UK

Nucleotide excision repair (NER) removes bulky DNA lesions andis thus crucial for the protection against environmental carcinogensand UV light exposure. Deficiencies in NER cause increased mutationrates and chromosomal aberrations. Current methods for studyingNER are mostly based on either quantitation of lesion removalor detection of repair DNA synthesis. Both have their limitations:lesion removal is inaccurate at very short times post-lesion,where the fraction of removal is low. Repair synthesis is difficultto apply to normally cycling cells due to the need to discriminaterepair from replicative DNA synthesis. To overcome these problemswe developed a method for analysis of NER based on detectionof transient single-stranded (ss) DNA stretches generated atthe nucleotide excision step. Cells are metabolically labelledwith BrdU, exposed to UV-irradiation and the ssDNA transientsgenerated during excision repair are detected using an anti-BrdUantibody. The method allows single-cell microscopic analysisof the distribution of DNA repair sites as well as kinetic analysisof the DNA repair response. Studies using various DNA repair-deficientcell lines indicate that the detection method integrates a numberof pre-synthesis nucleotide excision repair stages. Thus, assembledrepair sites can be detected even when they may not lead tocomplete resolution of the DNA lesion. Using this approach,we show that repair helicase-deficient cells differ from endonuclease-deficientcells.

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