A single amino acid substitution in DNA-PKcs explains the novel phenotype of the CHO mutant, XR-C2

doi:10.1093/nar/gkf625

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Nucleic Acids Research, 2002, Vol. 30, No. 23 5120-5128
© 2002 Oxford University Press

A single amino acid substitution in DNA-PKcs explains the novel phenotype of the CHO mutant, XR-C2

Timothy Woods, Wei Wang, Erin Convery, Abdellatif Errami¹, Malgorzata Z. Zdzienicka¹^,2 and Katheryn Meek^*

College of Veterinary Medicine, Department of Pathobiology and Diagnostic Investigation, Michigan State University, 350 FST, East Lansing, MI 48824, USA, ¹ Department of Radiation Genetics and Chemical Mutagenesis, Leiden University, Medical Center, Leiden, The Netherlands and ² Department of Molecular Cell Genetics, The Ludwil Rydygier University of Medical Sciences, Bydgoszcz, Poland

*To whom correspondence should be addressed. Tel: +1 517 432 9505; Fax: +1 517 353 9004; Email: kmeek{at}msu.edu

We recently described a CHO DSBR mutant belonging to the XRCC7complementation group (XR-C2) that has the interesting phenotypeof being radiosensitive, but having only a modest defect inVDJ recombination. This cell line expresses only slightly reducedlevels of DNA-PKcs but has undetectable DNA-PK activity. Limitedsequence analyses of DNA-PKcs transcripts from XR-C2 revealeda point mutation that results in an amino acid substitutionof glutamic acid for glycine six residues from the C-terminus.To determine whether this single substitution was responsiblefor the phenotype in XR-C2 cells, we introduced the mutationinto a DNA-PKcs expression vector. Whereas transfection of thisexpression vector significantly restores the VDJ recombinationdeficits in DNA-PKcs-deficient cells, radioresistance is notrestored. Thus, expression of this mutant form of DNA-PKcs inDNA-PKcs- deficient cells substantially recapitulates the phenotypeobserved in XR-C2, and we conclude that this single amino acidsubstitution is responsible for the non-homologous end joiningdeficits observed in XR-C2.

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