Article ID | Journal | Published Year | Pages | File Type |
---|---|---|---|---|
10823537 | DNA Repair | 2009 | 7 Pages |
Abstract
Ataxia oculomotor apraxia-1 (AOA1) is an autosomal recessive neurodegenerative disease that results from mutations of aprataxin (APTX). APTX associates with the DNA single- and double-strand break repair machinery and is able to remove AMP from 5â²-termini at DNA strand breaks in vitro. However, attempts to establish a DNA strand break repair defect in APTX-defective cells have proved conflicting and unclear. We reasoned that this may reflect that DNA strand breaks with 5â²-AMP represent only a minor subset of breaks induced in cells, and/or the availability of alternative mechanisms for removing AMP from 5â²-termini. Here, we have attempted to increase the dependency of chromosomal single- and double-strand break repair on aprataxin activity by slowing the rate of repair of 3â²-termini in aprataxin-defective neural cells, thereby increasing the likelihood that the 5â²-termini at such breaks become adenylated and/or block alternative repair mechanisms. To do this, we generated a mouse model in which APTX is deleted together with tyrosyl DNA phosphodiesterase (TDP1), an enzyme that repairs 3â²-termini at a subset of single-strand breaks (SSBs), including those with 3â²-topoisomerase-1 (Top1) peptide. Notably, the global rate of repair of oxidative and alkylation-induced SSBs was significantly slower in Tdp1â/â/Aptxâ/â double knockout quiescent mouse astrocytes compared with Tdp1â/â or Aptxâ/â single knockouts. In contrast, camptothecin-induced Top1-SSBs accumulated to similar levels in Tdp1â/â and Tdp1â/â/Aptxâ/â double knockout astrocytes. Finally, we failed to identify a measurable defect in double-strand break repair in Tdp1â/â, Aptxâ/â or Tdp1â/â/Aptxâ/â astrocytes. These data provide direct evidence for a requirement for aprataxin during chromosomal single-strand break repair in primary neural cells lacking Tdp1.
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Authors
Sherif F. El-Khamisy, Sachin Katyal, Poorvi Patel, Limei Ju, Peter J. McKinnon, Keith W. Caldecott,