Nucleotide sequence evidence for rapid genotypic shifts in the bovine mitochondrial DNA D-loop

Olivo, Paul D.; Walle, M J Van de; Laipis, Philip J.; Hauswirth, William W.

doi:10.1038/306400a0

Cited by 230 publications

(141 citation statements)

References 22 publications

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“…Although the present work has not addressed directly the question of whether fusion occurred between organelles carrying different mtDNAs, the most plausible hypothesis is that the lack of interaction between the two genomes reflected their physical segregation in separate organelles, i.e., absence of mitochondrial fusion. There is other evidence in the literature that supports the idea that two types of mtDNA originally located in separate organelles tend to remain segregated in mammalian cells, including the gradual elimination of HeLa cell mtDNA in hybrids of HeLa cells and fibroblasts (21,49) and the complete switch, in only one or a few generations, of mtDNA genotypes in Holstein cows (2,28,36). A model assuming that the unit of segregation of mammalian mtDNA is the organelle itself and that the rapidity of segregation of mitochondrial alleles within heteroplasmic oocytes is therefore influenced by whether the individual organelles themselves are homoplasmic or heteroplasmic (23) likewise argues in favor of the genetic independence of the individual mitochondria within a mammalian cell.…”

Section: Discussionmentioning

confidence: 90%

Complementation of mutant and wild-type human mitochondrial DNAs coexisting since the mutation event and lack of complementation of DNAs introduced separately into a cell within distinct organelles.

1994

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The rules that govern complementation of mutant and wild-type mitochondrial genomes in human cells were investigated under different experimental conditions. Among mitochondrial transformants derived from an individual affected by the MERRF (myoclonus epilepsy associated with ragged red fibers) encephalomyopathy and carrying in heteroplasmic form the mitochondrial tRNALYS mutation associated with that syndrome, normal protein synthesis and respiration was observed when the wild-type mitochondrial DNA exceeded 10% of the total complement. In these transformants, the protective effect of wild-type mitochondrial DNA was shown to involve interactions of the mutant and wild-type gene products. Very different results were obtained in experiments in which two mitochondrial DNAs carrying nonallelic disease-causing mutations were sequentially introduced within distinct organelles into the same human mitochondrial DNA-less (p°) cell. In transformants exhibiting different ratios of the two genomes, no evidence of cooperation between their products was observed, even 3 months after the introduction of the second mutation. These results pointed to the phenotypic independence of the two genomes. A similar conclusion was reached in experiments in which mitochondria carrying a chloramphenicol resistance-inducing mitochondrial DNA mutation were introduced into chloramphenicol-sensitive cells. A plausible interpretation of the different results obtained in the latter two sets of experiments, compared with the complementation behavior observed in the heteroplasmic MERRF transformants, is that in the latter, the mutant and wild-type genomes coexisted in the same organelles from the time of the mutation. This would imply that the way in which mitochondrial DNA is sorted among different organelles plays a fundamental role in determining the oxidative-phosphorylation phenotype in mammalian cells. These results have significant implications for mitochondrial genetics and for studies on the transmission and therapy of mitochondrial DNA-linked diseases.Despite the large number of studies on the expression of artificially produced mitochondrial DNA (mtDNA) mutations and the phenotype of somatic cell hybrids and cybrids, information on mitochondrial genome interactions in mammalian cells is still very limited. The dependence of such interactions on the distribution of the mtDNA molecules among the mitochondria, which changes continuously throughout division and, possibly, fusion of the organelles, and the difficulty of investigating mtDNA sorting in a cell account in part for the present lack of understanding of how much the mitochondrial genomes interact in mammalian cells. The recent discovery of a variety of mtDNA mutations associated with diseases in humans (47) and the growing evidence of accumulation of mtDNA mutations with aging in somatic tissues (12-14, 19, 43) have raised a number of questions about the occurrence and frequency of intermixing of mutant and wild-type mtDNA and/or their products within a cell and the role that co...

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Section: Discussionmentioning

confidence: 90%

Complementation of mutant and wild-type human mitochondrial DNAs coexisting since the mutation event and lack of complementation of DNAs introduced separately into a cell within distinct organelles.

1994

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“…Segregation also occurs before birth and has been involved in the rapid return to homoplasmy of heteroplasmic mtDNA molecules through what was called the genetic bottleneck [38]. It can theoretically take place at any step from the differentiation of primordial germinal cells, through their maturation into mature ovule, fecundation and embryogenesis.…”

Section: Segregation Of Mutations Through Generationsmentioning

confidence: 99%

Unsolved issues related to human mitochondrial diseases

et al. 2014

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Human mitochondrial diseases, defined as the diseases due to a mitochondrial oxidative phosphorylation defect, represent a large group of very diverse diseases with respect to phenotype and genetic causes. They present with many unsolved issues, the comprehensive analysis of which is beyond the scope of this review. We here essentially focus on the mechanisms underlying the diversity of targeted tissues, which is an important component of the large panel of these diseases phenotypic expression. The reproducibility of genotype/phenotype expression, the presence of modifying factors, and the potential causes for the restricted pattern of tissular expression are reviewed.Special emphasis is made on heteroplasmy, a specific feature of mitochondrial diseases, defined as the coexistence within the cell of mutant and wild type mitochondrial DNA molecules. Its existence permits unequal segregation during mitoses of the mitochondrial DNA populations and consequently heterogeneous tissue distribution of the mutation load. The observed tissue distributions of recurrent human mitochondrial DNA deleterious mutations are diverse but reproducible for a given mutation demonstrating that the segregation is not a random process. Its extent and mechanisms remain essentially unknown despite recent advances obtained in animal models.

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“…Considering the effect of rate variation among a small number of genes, it is not surprising that the analyses based on partial mitochondrial gene sequences may sometimes be biased. As a genetic marker, animal mitochondrial DNA (mtDNA) has distinct characteristics, such as relatively fast evolutionary rate, lack of recombination, and maternal inheritance (e.g., Brown et al, 1979;Olivio et al, 1983). One way of reducing the problems associated with molecular clock dating is to compare long DNA sequence data (e.g., Inoue et al, 2001aInoue et al, , 2003Yang and Yoder, 2003).…”

Section: Introductionmentioning

confidence: 99%

Mitochondrial molecular clocks and the origin of the major Otocephalan clades (Pisces: Teleostei): A new insight

Peng

Wang

et al. 2006

Gene

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Nucleotide sequence evidence for rapid genotypic shifts in the bovine mitochondrial DNA D-loop

Cited by 230 publications

References 22 publications

Complementation of mutant and wild-type human mitochondrial DNAs coexisting since the mutation event and lack of complementation of DNAs introduced separately into a cell within distinct organelles.

Complementation of mutant and wild-type human mitochondrial DNAs coexisting since the mutation event and lack of complementation of DNAs introduced separately into a cell within distinct organelles.

Unsolved issues related to human mitochondrial diseases

Mitochondrial molecular clocks and the origin of the major Otocephalan clades (Pisces: Teleostei): A new insight

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