| Literature DB >> 33437445 |
Franziska Trede1,2, Niels Kil2,3,4,5, James Stranks2,3,4,5, Andrew Jesse Connell6, Julia Fischer1,4,7, Julia Ostner3,4,5, Oliver Schülke3,4,5, Dietmar Zinner1,4,7, Christian Roos2,8.
Abstract
Microsatellite genotyping is an important genetic method for a number of research questions in biology. Given that the traditional fragment length analysis using polyacrylamide gel or capillary electrophoresis has several drawbacks, microsatellite genotyping-by-sequencing (GBS) has arisen as a promising alternative. Although GBS mitigates many of the problems of fragment length analysis, issues with allelic dropout and null alleles often remain due to mismatches in primer binding sites and unnecessarily long PCR products. This is also true for GBS in catarrhine primates where cross-species amplification of loci (often human derived) is common.We therefore redesigned primers for 45 microsatellite loci based on 17 available catarrhine reference genomes. Next, we tested them in singleplex and different multiplex settings in a panel of species representing all major lineages of Catarrhini and further validated them in wild Guinea baboons (Papio papio) using fecal samples.The final panel of 42 microsatellite loci can efficiently be amplified with primers distributed into three amplification pools.With our microsatellite panel, we provide a tool to universally genotype catarrhine primates via GBS from different sample sources in a cost- and time-efficient way, with higher resolution, and comparability among laboratories and species.Entities:
Keywords: Old World monkeys; apes; genotyping‐by‐sequencing; high‐throughput sequencing; simple tandem repeats
Year: 2020 PMID: 33437445 PMCID: PMC7790618 DOI: 10.1002/ece3.7069
Source DB: PubMed Journal: Ecol Evol ISSN: 2045-7758 Impact factor: 2.912