2011
DOI: 10.1111/j.1755-0998.2011.03056.x
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DNA barcoding meets molecular scatology: short mtDNA sequences for standardized species assignment of carnivore noninvasive samples

Abstract: Although species assignment of scats is important to study carnivore biology, there is still no standardized assay for the identification of carnivores worldwide, which would allow large-scale routine assessments and reliable cross-comparison of results. Here, we evaluate the potential of two short mtDNA fragments [ATP6 (126 bp) and cytochrome oxidase I gene (COI) (187 bp)] to serve as standard markers for the Carnivora. Samples of 66 species were sequenced for one or both of these segments. Alignments were co… Show more

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Cited by 75 publications
(61 citation statements)
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References 88 publications
(158 reference statements)
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“…The neighbor-joining-tree recovered these three jaguar samples within the group of Panthera onca (Figure 1), reinforcing that the method used was able to correctly identify the species who deposited the faeces collected. The ATP6 and CytB gene have been previously used for felid identification (Chaves et al 2012, Miotto et al 2014, Wultsch et al 2016, and proved to be a powerful molecular marker for this group of carnivores.…”
Section: Resultsmentioning
confidence: 99%
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“…The neighbor-joining-tree recovered these three jaguar samples within the group of Panthera onca (Figure 1), reinforcing that the method used was able to correctly identify the species who deposited the faeces collected. The ATP6 and CytB gene have been previously used for felid identification (Chaves et al 2012, Miotto et al 2014, Wultsch et al 2016, and proved to be a powerful molecular marker for this group of carnivores.…”
Section: Resultsmentioning
confidence: 99%
“…A CytB primer pair developed by Farrel et al (2001) was used to amplify a fragment of the Cytochrome B gene, and the ATP6-DF3; ATP6-DR2 primer pair (Chaves et al 2012) was used to amplify a fragment of the ATP6 gene, following the respective PCR protocols given by the already cited authors. All PCRs were carried out using a Veriti 96 Well Thermal Cycler (Applied Biosystems) and tissue sample DNA as a positive control.…”
Section: Molecular Species Identificationmentioning
confidence: 99%
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“…PCR conditions for species identification can be found in Chaves et al (2012). PCR conditions for microsatellite amplification and sex ID were as follows.…”
Section: Appendix 1 Pcr Conditionsmentioning
confidence: 99%
“…For species identification, we amplified a 126-bp fragment of the mitochondrial gene ATP6 by polymerase chain reaction (PCR) using primers ATP6-DF3 and ATP6-DR1 following conditions from Chaves et al [36]. PCR products were sequenced on an Applied Biosystems 3730xl DNA analyzer, and resulting sequences were compared to reference sequences using the online tool DNA Surveillance Carnivora [36].…”
Section: Dna Extraction and Species Identificationmentioning
confidence: 99%