| Literature DB >> 28753409 |
J Vierna1, J Doña2, A Vizcaíno1, D Serrano3, R Jovani2.
Abstract
High-throughput DNA barcoding has become essential in ecology and evolution, but some technical questions still remain. Increasing the number of PCR cycles above the routine 20-30 cycles is a common practice when working with old-type specimens, which provide little amounts of DNA, or when facing annealing issues with the primers. However, increasing the number of cycles can raise the number of artificial mutations due to polymerase errors. In this work, we sequenced 20 COI libraries in the Illumina MiSeq platform. Libraries were prepared with 40, 45, 50, 55, and 60 PCR cycles from four individuals belonging to four species of four genera of cephalopods. We found no relationship between the number of PCR cycles and the number of mutations despite using a nonproofreading polymerase. Moreover, even when using a high number of PCR cycles, the resulting number of mutations was low enough not to be an issue in the context of high-throughput DNA barcoding (but may still remain an issue in DNA metabarcoding due to chimera formation). We conclude that the common practice of increasing the number of PCR cycles should not negatively impact the outcome of a high-throughput DNA barcoding study in terms of the occurrence of point mutations.Keywords: COI; DNA barcoding; Illumina; codage à barres de l’ADN; librairie; library; mutations; non-proofreading polymerase; polymérase sans activité exonucléase 3′→5′
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Year: 2017 PMID: 28753409 DOI: 10.1139/gen-2017-0081
Source DB: PubMed Journal: Genome ISSN: 0831-2796 Impact factor: 2.166