Journal
AGING CELL
Volume 8, Issue 4, Pages 502-506Publisher
WILEY
DOI: 10.1111/j.1474-9726.2009.00484.x
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Funding
- Medical Research Council [G0700718] Funding Source: researchfish
- Medical Research Council [G0700718] Funding Source: Medline
- NIA NIH HHS [R03 AG035223, R01AG019787, R03 AG035223-02, R01 AG019787] Funding Source: Medline
- NIMH NIH HHS [R01 MH085801] Funding Source: Medline
- NINDS NIH HHS [R01 NS058988-05, R01 NS058988, R03 NS053840-02, R01 NS058988-04, 1R01NS058988, R03 NS053840] Funding Source: Medline
- MRC [G0700718] Funding Source: UKRI
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P>Deletions in mitochondrial DNA (mtDNA) have long been suspected to be involved in mammalian aging, but their role remains controversial. Recent research has demonstrated that relatively higher levels of mtDNA deletions correlate with premature aging in mtDNA mutator mice, which led to the conclusion that premature aging in these mice is driven by mtDNA deletions. However, it is reported here that the absolute level of deletions in mutator mice is quite low, especially when compared with the level of point mutations in these mice. It is thus argued that the available data are insufficient to conclude that mtDNA mutations drive premature aging in mtDNA mutator mice. It remains possible that clonal expansion of mtDNA deletions may result in sufficiently high levels to play a role in age-related dysfunction in some cells, but assessing this possibility will require studies of the distribution of these deletions among different cell types and in individual cells.
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