Survival, mutagenesis, and host cell reactivation in a Chinese hamster ovary cell ERCC1 knock-out mutant |
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| Authors: | Rolig, Rhonda L. Layher, Susan K. Santi, Barbara Adair, Gerald M. Gu, Feng Rainbow, Andrew J. Nairn, Rodney S. |
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| Affiliation: | 1Department of Carcinogenesis, University of Texas M.D.Anderson Cancer Center, Science Park-Research Division PO Box 389, Smithville, TX 78957, USA 2department of Biology, McMaster University Hamilton, Ontario L8S 4K1, Canada 3 Present address: BDIS, 2530 Qume Drive, San Jose, California 95131, USA |
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| Abstract: | Positive selection-negative selection gene targeting was usedto disrupt the nucleotide excision repair gene ERCC1 in a Chinesehamster ovary cell line, CHO-K1. Southern and Northern analysisshowed that a cell clone isolated by this targeting approach,CHO-7-27, had an ERCC1 gene structure consistent with targeteddisruption of ERCC1 exon V, and did not express ERCC1 mRNA.CHO-7-27 was further characterized with respect to UV and mitomycinC sensitivities, and was shown to exhibit severe mutagen sensitivityphenotypes consistent with those of other CHO cell ERCC1 mutants.Mutation frequency experiments showed that CHO-7-27 was UV-hypermutableat the hypoxanthine-guanine phosphoribosyltransferase locus.Experiments assessing host cell reactivation of viral DNA synthesisfor UV-irradiated adenovirus showed that CHO7-27 exhibited aseverely deficient HCR phenotype similar to that of UV20 cells.Our results demonstrate that CHOK1 cells are hemizygous forthe ERCC1 gene, and show that the comparatively mild mutagensensitivities and lack of severely deficient HCR phenotypesof conventionally derived CHO-K1 ERCC1 mutants, in contrastto the severe phenotypes of CHO-AA8-derived mutants, are notdue to any intrinsic genetic differences between CHO-K1 andCHO-AA8 parental cell lines. 4To whom correspondence should be addressed |
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