Assessing genotyping errors in mammalian museum study skins using high-throughput genotyping-by-sequencing

被引:5
作者
Yuan, Stella C. [1 ]
Malekos, Eric [2 ]
Hawkins, Melissa T. R. [1 ,3 ,4 ]
机构
[1] Humboldt State Univ, Dept Biol Sci, 1 Harpst St, Arcata, CA 95521 USA
[2] Humboldt State Univ, Dept Math, 1 Harpst St, Arcata, CA 95521 USA
[3] Natl Museum Nat Hist, Dept Vertebrate Zool, Div Mammals, 10th & Constitut Ave NW, Washington, DC 20560 USA
[4] George Mason Univ, Dept Biol, 4400 Univ Dr, Fairfax, VA 22030 USA
关键词
Microsatellite; Museum specimens; Degraded DNA; Population genetics; SSRseq; NORTHERN FLYING SQUIRRELS; ANCIENT DNA; MICROSATELLITE MARKERS; PIPELINE; HISTORY; SAMPLES; LOCI;
D O I
10.1007/s12686-021-01213-8
中图分类号
X176 [生物多样性保护];
学科分类号
090705 ;
摘要
The use of museum specimens held in natural history repositories for population and conservation genetic research is increasing in tandem with the use of massively parallel sequencing technologies. Short Tandem Repeats (STRs), or microsatellite loci, are commonly used genetic markers in wildlife and population genetic studies. However, they traditionally suffered from a host of issues including length homoplasy, high costs, low throughput, and difficulties in reproducibility across laboratories. Massively parallel sequencing technologies can address these problems, but the incorporation of museum specimen derived DNA suffers from significant fragmentation and exogenous DNA contamination. Combatting these issues requires extra measures of stringency in the lab and during data analysis, yet there have not been any high-throughput sequencing studies evaluating microsatellite allelic dropout from museum specimen extracted DNA. In this study, we evaluate genotyping errors derived from mammalian museum skin DNA extracts for previously characterized microsatellites across PCR replicates utilizing high-throughput sequencing. We found it useful to classify samples based on DNA concentration, which determined the rate by which genotypes were accurately recovered. Longer microsatellites performed worse in all museum specimens. Allelic dropout rates across loci were dependent on sample quantity, with high concentration museum specimens performing as well and recovering quality metrics nearly as high as the frozen tissue sample. Based on our results, we provide a set of best practices for quality assurance and incorporation of reliable genotypes from museum specimens.
引用
收藏
页码:303 / 317
页数:15
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