Molecular-based approaches for species identification and delimitation strongly rely, in terms of universality and efficiency, on the selected markers. Conventionally, when adopting a DNA barcoding approach to discriminate (or identify) metazoans species, the marker choice falls on the 658 base pair region at the 5MODIFIER LETTER PRIME end of the mitochondrial COI gene. However, a growing number of studies suggest to use alternative and more variable genetic regions, even from the same gene, such as the 3MODIFIER LETTER PRIME end of the COI. In this work, we compared the identification performance of the 5MODIFIER LETTER PRIME and 3MODIFIER LETTER PRIME end COI regions on a large sequence dataset of odonate species, an order of arthropods among the most studied in terms of conservation importance for aquatic ecosystems. The genetic datasets comprised a total of 236 specimens, 113 species, 51 genera and 12 families spanning the two odonate suborders Zygoptera and Anisoptera, and were analysed under an integrative multiple approach including descriptive statistics and variability of the sequences, phylogenetic reconstructions, DNA-based species delimitations, genetic distances, identification of diagnostic characters and saturation plots. All analyses were congruent in recovering the COI-3MODIFIER LETTER PRIME region to be slightly more variable than the COI-5MODIFIER LETTER PRIME one, and both regions showed a saturation of transversion at the third codon position. However, phylogenetic reconstructions, genetic distances, and diagnostic characters identification resulted in a similar discrimination power for the two COI regions. Therefore, the COI-3MODIFIER LETTER PRIME region does not add much information to the standard COI-5MODIFIER LETTER PRIME barcode region, which has in turn largely been demonstrated to successfully delineate invertebrate communities through DNA and eDNA metabarcoding, and to have a much more extensive taxonomic coverage in public databases. Overall, the DNA barcoding inventory assembled in this study will provide valuable insights into the systematics and conservation of many odonate species with implications for future DNA and eDNA monitoring-based studies.
Maggioni, D., Assandri, G., Ramazzotti, F., Magnani, D., Pellegrino, I., Valsecchi, E., et al. (2021). Differential genetic variability at two mtDNA COI regions does not imply mismatches in Odonata molecular identification performances. THE EUROPEAN ZOOLOGICAL JOURNAL, 88(1), 425-435 [10.1080/24750263.2021.1896795].
Differential genetic variability at two mtDNA COI regions does not imply mismatches in Odonata molecular identification performances
Maggioni, D.Primo
;Valsecchi, E.;Galimberti, A.
Ultimo
2021
Abstract
Molecular-based approaches for species identification and delimitation strongly rely, in terms of universality and efficiency, on the selected markers. Conventionally, when adopting a DNA barcoding approach to discriminate (or identify) metazoans species, the marker choice falls on the 658 base pair region at the 5MODIFIER LETTER PRIME end of the mitochondrial COI gene. However, a growing number of studies suggest to use alternative and more variable genetic regions, even from the same gene, such as the 3MODIFIER LETTER PRIME end of the COI. In this work, we compared the identification performance of the 5MODIFIER LETTER PRIME and 3MODIFIER LETTER PRIME end COI regions on a large sequence dataset of odonate species, an order of arthropods among the most studied in terms of conservation importance for aquatic ecosystems. The genetic datasets comprised a total of 236 specimens, 113 species, 51 genera and 12 families spanning the two odonate suborders Zygoptera and Anisoptera, and were analysed under an integrative multiple approach including descriptive statistics and variability of the sequences, phylogenetic reconstructions, DNA-based species delimitations, genetic distances, identification of diagnostic characters and saturation plots. All analyses were congruent in recovering the COI-3MODIFIER LETTER PRIME region to be slightly more variable than the COI-5MODIFIER LETTER PRIME one, and both regions showed a saturation of transversion at the third codon position. However, phylogenetic reconstructions, genetic distances, and diagnostic characters identification resulted in a similar discrimination power for the two COI regions. Therefore, the COI-3MODIFIER LETTER PRIME region does not add much information to the standard COI-5MODIFIER LETTER PRIME barcode region, which has in turn largely been demonstrated to successfully delineate invertebrate communities through DNA and eDNA metabarcoding, and to have a much more extensive taxonomic coverage in public databases. Overall, the DNA barcoding inventory assembled in this study will provide valuable insights into the systematics and conservation of many odonate species with implications for future DNA and eDNA monitoring-based studies.
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