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Article Abstract

Cephalopods are pivotal components of marine food webs, but biodiversity studies are hampered by challenges to sample these agile marine molluscs. Metabarcoding of environmental DNA (eDNA) is a potentially powerful technique to study oceanic cephalopod biodiversity and distribution but has not been applied thus far. We present a novel universal primer pair for metabarcoding cephalopods from eDNA, (Forward: 5'-CGC GGC GCT ACA TAT TAG AC-3', Reverse: 5'-GCA CTT AAC CGA CCG TCG AC-3'). The primer pair targets the hypervariable region V2 of the nuclear 18S rRNA gene and amplifies a relatively short target sequence of approximately 200 bp in order to allow the amplification of degraded DNA. tests on a reference database and empirical tests on DNA extracts from cephalopod tissue estimate that 44-66% of cephalopod species, corresponding to about 310-460 species, can be amplified and identified with this primer pair. A multi-marker approach with the novel and two previously published cephalopod mitochondrial 16S rRNA primer sets targeting the same region (Jarman . 2006 , 268-271; Peters . 2015 , 1428-1439) is estimated to amplify and identify 89% of all cephalopod species, of which an estimated 19% can only be identified by . All sequences obtained with were submitted to GenBank, resulting in new 18S rRNA sequences for 13 cephalopod taxa.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8074623PMC
http://dx.doi.org/10.1098/rsos.201388DOI Listing

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