A method for multiplexed full-length single-molecule sequencing of the human mitochondrial genome

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作者
Ieva Keraite
Philipp Becker
Davide Canevazzi
Cristina Frias-López
Marc Dabad
Raúl Tonda-Hernandez
Ida Paramonov
Matthew John Ingham
Isabelle Brun-Heath
Jordi Leno
Anna Abulí
Elena Garcia-Arumí
Simon Charles Heath
Marta Gut
Ivo Glynne Gut
机构
[1] The Barcelona Institute of Science and Technology (BIST),CNAG
[2] Institute for Research in Biomedicine (IRB Barcelona) - The Barcelona Institute of Science and Technology (BIST),CRG, Centre for Genomic Regulation (CRG)
[3] Joint IRB-BSC Program in Computational Biology,Department of Clinical and Molecular Genetics and Rare Disease
[4] Hospital Universitari Vall d’Hebron,undefined
[5] Medicine Genetics Group,undefined
[6] VHIR,undefined
[7] Hospital Universitari Vall d’Hebron,undefined
[8] Research Group on Neuromuscular and Mitochondrial Disorders,undefined
[9] VHIR,undefined
[10] Hospital Universitari Vall d’Hebron,undefined
[11] Centro de Investigación Biomédica en Red de Enfermedades Raras (CIBERER),undefined
[12] Instituto de Salud Carlos III,undefined
[13] Universitat Pompeu Fabra,undefined
[14] Qiagen,undefined
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摘要
Methods to reconstruct the mitochondrial DNA (mtDNA) sequence using short-read sequencing come with an inherent bias due to amplification and mapping. They can fail to determine the phase of variants, to capture multiple deletions and to cover the mitochondrial genome evenly. Here we describe a method to target, multiplex and sequence at high coverage full-length human mitochondrial genomes as native single-molecules, utilizing the RNA-guided DNA endonuclease Cas9. Combining Cas9 induced breaks, that define the mtDNA beginning and end of the sequencing reads, as barcodes, we achieve high demultiplexing specificity and delineation of the full-length of the mtDNA, regardless of the structural variant pattern. The long-read sequencing data is analysed with a pipeline where our custom-developed software, baldur, efficiently detects single nucleotide heteroplasmy to below 1%, physically determines phase and can accurately disentangle complex deletions. Our workflow is a tool for studying mtDNA variation and will accelerate mitochondrial research.
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