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Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens

Laboratory techniques for high‐throughput sequencing have enhanced our ability to generate DNA sequence data from millions of natural history specimens collected prior to the molecular era, but remain poorly tested at shallower evolutionary time scales. Hybridization capture using restriction site‐a...

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Autores principales: Linck, Ethan B., Hanna, Zachary R., Sellas, Anna, Dumbacher, John P.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley and Sons Inc. 2017
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5496524/
https://www.ncbi.nlm.nih.gov/pubmed/28690805
http://dx.doi.org/10.1002/ece3.3065
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author Linck, Ethan B.
Hanna, Zachary R.
Sellas, Anna
Dumbacher, John P.
author_facet Linck, Ethan B.
Hanna, Zachary R.
Sellas, Anna
Dumbacher, John P.
author_sort Linck, Ethan B.
collection PubMed
description Laboratory techniques for high‐throughput sequencing have enhanced our ability to generate DNA sequence data from millions of natural history specimens collected prior to the molecular era, but remain poorly tested at shallower evolutionary time scales. Hybridization capture using restriction site‐associated DNA probes (hyRAD) is a recently developed method for population genomics with museum specimens. The hyRAD method employs fragments produced in a restriction site‐associated double digestion as the basis for probes that capture orthologous loci in samples of interest. While promising in that it does not require a reference genome, hyRAD has yet to be applied across study systems in independent laboratories. Here, we provide an independent assessment of the effectiveness of hyRAD on both fresh avian tissue and dried tissue from museum specimens up to 140 years old and investigate how variable quantities of input DNA affect sequencing, assembly, and population genetic inference. We present a modified bench protocol and bioinformatics pipeline, including three steps for detection and removal of microbial and mitochondrial DNA contaminants. We confirm that hyRAD is an effective tool for sampling thousands of orthologous SNPs from historic museum specimens to describe phylogeographic patterns. We find that modern DNA performs significantly better than historical DNA better during sequencing but that assembly performance is largely equivalent. We also find that the quantity of input DNA predicts %GC content of assembled contiguous sequences, suggesting PCR bias. We caution against sampling schemes that include taxonomic or geographic autocorrelation across modern and historic samples.
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spelling pubmed-54965242017-07-07 Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens Linck, Ethan B. Hanna, Zachary R. Sellas, Anna Dumbacher, John P. Ecol Evol Original Research Laboratory techniques for high‐throughput sequencing have enhanced our ability to generate DNA sequence data from millions of natural history specimens collected prior to the molecular era, but remain poorly tested at shallower evolutionary time scales. Hybridization capture using restriction site‐associated DNA probes (hyRAD) is a recently developed method for population genomics with museum specimens. The hyRAD method employs fragments produced in a restriction site‐associated double digestion as the basis for probes that capture orthologous loci in samples of interest. While promising in that it does not require a reference genome, hyRAD has yet to be applied across study systems in independent laboratories. Here, we provide an independent assessment of the effectiveness of hyRAD on both fresh avian tissue and dried tissue from museum specimens up to 140 years old and investigate how variable quantities of input DNA affect sequencing, assembly, and population genetic inference. We present a modified bench protocol and bioinformatics pipeline, including three steps for detection and removal of microbial and mitochondrial DNA contaminants. We confirm that hyRAD is an effective tool for sampling thousands of orthologous SNPs from historic museum specimens to describe phylogeographic patterns. We find that modern DNA performs significantly better than historical DNA better during sequencing but that assembly performance is largely equivalent. We also find that the quantity of input DNA predicts %GC content of assembled contiguous sequences, suggesting PCR bias. We caution against sampling schemes that include taxonomic or geographic autocorrelation across modern and historic samples. John Wiley and Sons Inc. 2017-05-23 /pmc/articles/PMC5496524/ /pubmed/28690805 http://dx.doi.org/10.1002/ece3.3065 Text en © 2017 The Authors. Ecology and Evolution published by John Wiley & Sons Ltd. This is an open access article under the terms of the Creative Commons Attribution (http://creativecommons.org/licenses/by/4.0/) License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited.
spellingShingle Original Research
Linck, Ethan B.
Hanna, Zachary R.
Sellas, Anna
Dumbacher, John P.
Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title_full Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title_fullStr Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title_full_unstemmed Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title_short Evaluating hybridization capture with RAD probes as a tool for museum genomics with historical bird specimens
title_sort evaluating hybridization capture with rad probes as a tool for museum genomics with historical bird specimens
topic Original Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5496524/
https://www.ncbi.nlm.nih.gov/pubmed/28690805
http://dx.doi.org/10.1002/ece3.3065
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