2019
DOI: 10.1002/ece3.4960
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Application of a SSR‐GBS marker system on investigation of European Hedgehog species and their hybrid zone dynamics

Abstract: By applying second‐generation sequencing technologies to microsatellite genotyping, sequence information is produced which can result in high‐resolution population genetics analysis populations and increased replicability between runs and laboratories. In the present study, we establish an approach to study the genetic structure patterns of two European hedgehog species Erinaceaus europaeus and E. roumanicus . These species are usually associated with human settlem… Show more

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Cited by 56 publications
(75 citation statements)
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“…Genomic DNA extraction was conducted using magnetic beads based on the MagSi-DNA Vegetal kit (MagnaMedics, Geleen, Netherlands) and a magnetic separator, SL-MagSep96 (Steinbrenner, Germany) [27,30]. We used microsatellite markers [27], to which we added 15 extra primers ( Table 2, see also Additional file 1: Table S3).…”
Section: Genotypingmentioning
confidence: 99%
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“…Genomic DNA extraction was conducted using magnetic beads based on the MagSi-DNA Vegetal kit (MagnaMedics, Geleen, Netherlands) and a magnetic separator, SL-MagSep96 (Steinbrenner, Germany) [27,30]. We used microsatellite markers [27], to which we added 15 extra primers ( Table 2, see also Additional file 1: Table S3).…”
Section: Genotypingmentioning
confidence: 99%
“…The raw sequence data were deposited in the GenBank, sequence read archive database (SRA) under the project PRJNA550300 with the accession numbers, SRR9587388 to SRR9587270. Sequences generated by Illumina, were subsequently quality checked and controlled, which were later used for alleles calling as described in [27,30] using the scripts from the SSR-GBS pipeline (https://github.com/mcurto/SSR-GBS-pipeline). The resulting codominant matrix and information for which sequences correspond to each allele can be found in the Additional file 2 (see the file named "Second_additional fileAllelesList & matrix_").For subsequent analyses, all loci and samples with missing genotypes ≥50% were excluded, leaving a total number of 40 markers (Additional file 1: Tables S1, S3).…”
Section: Genotypingmentioning
confidence: 99%
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“…On Sanger sequence‐based DNA barcoding, longer regions are collected (up to 800 bp), and consequently, these were chosen for pollen barcoding (CBOL Plant Working Group, ). Because the length for Illumina amplicon sequencing cannot exceed 500 bp (Curto et al ., ), mostly the chloroplast region rbcl and the ribosomal DNA marker ITS are preferably used (e.g. Richardson et al ., ; Bell et al ., 2017; Suchan et al ., ).…”
Section: Discussionmentioning
confidence: 99%
“…Paired reads were merged using pear (Zhang et al ., ) and amplification primers were trimmed using script 1 from Curto et al . (). The resulting reads were dereplicated and blast ed against all Spermatophyta chloroplast sequences present in GenBank.…”
Section: Methodsmentioning
confidence: 97%