Complete vertebrate mitogenomes reveal widespread gene duplications and repeats

Author:

Formenti GiulioORCID,Rhie ArangORCID,Balacco JenniferORCID,Haase BettinaORCID,Mountcastle Jacquelyn,Fedrigo OlivierORCID,Brown SamaraORCID,Capodiferro MarcoORCID,Al-Ajli Farooq O.ORCID,Ambrosini RobertoORCID,Houde PeterORCID,Koren SergeyORCID,Oliver Karen,Smith MichelleORCID,Skelton Jason,Betteridge Emma,Dolucan Jale,Corton CraigORCID,Bista IlianaORCID,Torrance JamesORCID,Tracey AlanORCID,Wood JonathanORCID,Uliano-Silva MarcelaORCID,Howe KerstinORCID,McCarthy ShaneORCID,Winkler Sylke,Kwak WooriORCID,Korlach JonasORCID,Fungtammasan ArkarachaiORCID,Fordham Daniel,Costa Vania,Mayes Simon,Chiara MatteoORCID,Horner David S.ORCID,Myers EugeneORCID,Durbin RichardORCID,Achilli AlessandroORCID,Braun Edward L.ORCID,Phillippy Adam M.ORCID,Jarvis Erich D.ORCID,

Abstract

AbstractModern sequencing technologies should make the assembly of the relatively small mitochondrial genomes an easy undertaking. However, few tools exist that address mitochondrial assembly directly. As part of the Vertebrate Genomes Project (VGP) we have developed mitoVGP, a fully automated pipeline for similarity-based identification of mitochondrial reads and de novo assembly of mitochondrial genomes that incorporates both long (>10 kbp, PacBio or Nanopore) and short (100-300 bp, Illumina) reads. Our pipeline led to successful complete mitogenome assemblies of 100 vertebrate species of the VGP. We have observed that tissue type and library size selection have considerable impact on mitogenome sequencing and assembly. Comparing our assemblies to purportedly complete reference mitogenomes based on short-read sequencing, we have identified errors, missing sequences, and incomplete genes in those references, particularly in repeat regions. Our assemblies have also identified novel gene region duplications, shedding new light on mitochondrial genome evolution and organization.

Publisher

Cold Spring Harbor Laboratory

Reference67 articles.

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