Accurate estimation of 5-methylcytosine in mammalian mitochondrial DNA

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作者
Shigeru Matsuda
Takehiro Yasukawa
Yuriko Sakaguchi
Kenji Ichiyanagi
Motoko Unoki
Kazuhito Gotoh
Kei Fukuda
Hiroyuki Sasaki
Tsutomu Suzuki
Dongchon Kang
机构
[1] Kyushu University,Department of Clinical Chemistry and Laboratory Medicine, Graduate School of Medical Sciences
[2] The University of Tokyo,Department of Chemistry and Biotechnology, Graduate School of Engineering
[3] Kyushu University,Division of Epigenomics and Development, Medical Institute of Bioregulation
[4] Nagoya University,Laboratory of Genome and Epigenome Dynamics, Department of Applied Molecular Biosciences, Graduate School of Bioagricultural Sciences
[5] Furo-cho,undefined
[6] Cellular Memory Laboratory,undefined
[7] RIKEN,undefined
[8] 2-1 Hirosawa,undefined
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Whilst 5-methylcytosine (5mC) is a major epigenetic mark in the nuclear DNA in mammals, whether or not mitochondrial DNA (mtDNA) receives 5mC modification remains controversial. Herein, we exhaustively analysed mouse mtDNA using three methods that are based upon different principles for detecting 5mC. Next-generation bisulfite sequencing did not give any significant signatures of methylation in mtDNAs of liver, brain and embryonic stem cells (ESCs). Also, treatment with methylated cytosine-sensitive endonuclease McrBC resulted in no substantial decrease of mtDNA band intensities in Southern hybridisation. Furthermore, mass spectrometric nucleoside analyses of highly purified liver mtDNA preparations did not detect 5-methyldeoxycytidine at the levels found in the nuclear DNA but at a range of only 0.3–0.5% of deoxycytidine. Taken together, we propose that 5mC is not present at any specific region(s) of mtDNA and that levels of the methylated cytosine are fairly low, provided the modification occurs. It is thus unlikely that 5mC plays a universal role in mtDNA gene expression or mitochondrial metabolism.
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