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Volume 38 Issue 4
Apr.  2011
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Toward genetic transformation of mitochondria in mammalian cells using a recoded drug-resistant selection marker

doi: 10.1016/j.jgg.2011.03.005
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  • Corresponding author: E-mail address: youngyoon97@gmail.com (Young Geol Yoon)
  • Received Date: 2010-12-10
  • Accepted Date: 2011-03-10
  • Rev Recd Date: 2011-03-07
  • Available Online: 2011-03-23
  • Publish Date: 2011-04-20
  • Due to technical difficulties, the genetic transformation of mitochondria in mammalian cells is still a challenge. In this report, we described our attempts to transform mammalian mitochondria with an engineered mitochondrial genome based on selection using a drug resistance gene. Because the standard drug-resistant neomycin phosphotransferase confers resistance to high concentrations of G418 when targeted to the mitochondria, we generated a recoded neomycin resistance gene that uses the mammalian mitochondrial genetic code to direct the synthesis of this protein in the mitochondria, but not in the nucleus (mitochondrial version). We also generated a universal version of the recoded neomycin resistance gene that allows synthesis of the drug-resistant proteins both in the mitochondria and nucleus. When we transfected these recoded neomycin resistance genes that were incorporated into the mouse mitochondrial genome clones into mouse tissue culture cells by electroporation, no DNA constructs were delivered into the mitochondria. We found that the universal version of the recoded neomycin resistance gene was expressed in the nucleus and thus conferred drug resistance to G418 selection, while the synthetic mitochondrial version of the gene produced no background drug-resistant cells from nuclear transformation. These recoded synthetic drug-resistant genes could be a useful tool for selecting mitochondrial genetic transformants as a precise technology for mitochondrial transformation is developed.
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