Molecular cloning of the human XRCC1 gene, which corrects defective DNA strand break repair and sister chromatid exchange.

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Mol Cell Biol. 1990 December; 10(12): 6160-6171

Molecular cloning of the human XRCC1 gene, which corrects defective DNA strand break repair and sister chromatid exchange.

L H Thompson, K W Brookman, N J Jones, S A Allen and A V Carrano

Biomedical Sciences Division, Lawrence Livermore National Laboratory, Livermore, California 94550.

ABSTRACT

We describe the cloning and function of the human XRCC1 gene,which is the first mammalian gene isolated that affects cellularsensitivity to ionizing radiation. The CHO mutant EM9 has 10-fold-highersensitivity to ethyl methanesulfonate, 1.8-fold-higher sensitivityto ionizing radiation, a reduced capacity to rejoin single-strandDNA breaks, and a 10-fold-elevated level of sister chromatidexchange compared with the CHO parental cells. The complementinghuman gene was cloned from a cosmid library of a tertiary transformant.Two cosmid clones produced transformants that showed approximately100% correction of the repair defect in EM9 cells, as determinedby the kinetics of strand break repair, cell survival, and thelevel of sister chromatid exchange. A nearly full-length cloneobtained from the pcD2 human cDNA expression library gave approximately80% correction of EM9, as determined by the level of sisterchromatid exchange. Based on an analysis of the nucleotide sequenceof the cDNA insert compared with that of the 5' end of the genefrom a cosmid clone, the cDNA clone appeared to be missing approximately100 bp of transcribed sequence, including 26 nucleotides ofcoding sequence. The cDNA probe detected a single transcriptof approximately 2.2 kb in HeLa polyadenylated RNA by Northern(RNA) blot hybridization. From the open reading frame and thepositions of likely start sites for transcription and translation,the size of the putative XRCC1 protein is 633 amino acids (69.5kDa). The size of the XRCC1 gene is 33 kb, as determined bylocalizing the endpoints on a restriction endonuclease sitemap of one cosmid clone. The deduced amino acid sequence didnot show significant homology with any protein in the proteinsequence data bases examined.

Mol Cell Biol. 1990 December; 10(12): 6160-6171

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