4.8 Article

Stable heteroplasmy at the single-cell level is facilitated by intercellular exchange of mtDNA

Journal

NUCLEIC ACIDS RESEARCH
Volume 43, Issue 4, Pages 2177-2187

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkv052

Keywords

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Funding

  1. National Institutes of Health (NIH) [1R21HG007394-01]
  2. Tisch Cancer Institute (TCI)
  3. A developmental award from the TCI
  4. pilot grant from the Venture Capital Research Funding Program of Children's Environmental Health Center (CEHC) at Mount Sinai funded several experiments
  5. National Cancer Institute (NCI)
  6. Breast Cancer Research foundation
  7. NIH [1R21HG007394-01]

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Eukaryotic cells carry two genomes, nuclear (nDNA) and mitochondrial (mtDNA), which are ostensibly decoupled in their replication, segregation and inheritance. It is increasingly appreciated that heteroplasmy, the occurrence of multiple mtDNA haplotypes in a cell, plays an important biological role, but its features are not well understood. Accurately determining the diversity of mtDNA has been difficult, due to the relatively small amount of mtDNA in each cell (<1% of the total DNA), the intercellular variability of mtDNA content and mtDNA pseudogenes (Numts) in nDNA. To understand the nature of heteroplasmy, we developed Mseek, a novel technique to purify and sequence mtDNA. Mseek yields high purity (>90%) mtDNA and its ability to detect rare variants is limited only by sequencing depth, providing unprecedented sensitivity and specificity. Using Mseek, we confirmed the ubiquity of heteroplasmy by analyzing mtDNA from a diverse set of cell lines and human samples. Applying Mseek to colonies derived fromsingle cells, we find heteroplasmy is stably maintained in individual daughter cells over multiple cell divisions. We hypothesized that the stability of heteroplasmy could be facilitated by intercellular exchange of mtDNA. We explicitly demonstrate this exchange by co-culturing cell lines with distinct mtDNA haplotypes. Our results shed newlight on themaintenance of heteroplasmy and provide a novel platform to investigate features of heteroplasmy in normal and diseased states.

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