A Target Capture-Based Method to Estimate Ploidy From Herbarium Specimens

Juan Viruel; María Conejero; Oriane Hidalgo; Lisa Pokorny; Robyn F Powell; Félix Forest; Michael B Kantar; Marybel Soto Gomez; Sean W Graham; Barbara Gravendeel; Paul Wilkin; Ilia J Leitch

doi:10.3389/fpls.2019.00937

A Target Capture-Based Method to Estimate Ploidy From Herbarium Specimens

Front Plant Sci. 2019 Jul 24:10:937. doi: 10.3389/fpls.2019.00937. eCollection 2019.

Authors

Juan Viruel¹, María Conejero¹, Oriane Hidalgo^{1

2}, Lisa Pokorny¹, Robyn F Powell¹, Félix Forest¹, Michael B Kantar³, Marybel Soto Gomez^{4

5}, Sean W Graham^{4

5}, Barbara Gravendeel^{6

7

8}, Paul Wilkin¹, Ilia J Leitch¹

Affiliations

¹ Royal Botanic Gardens, Kew, Richmond, United Kingdom.
² Laboratori de Botànica, Facultat de Farmàcia i Ciències de l'Alimentació, Universitat de Barcelona, Barcelona, Spain.
³ Department of Tropical Plant and Soil Sciences, University of Hawai'i at Mânoa, Honolulu, HI, United States.
⁴ Department of Botany, University of British Columbia, Vancouver, BC, Canada.
⁵ UBC Botanical Garden & Centre for Plant Research, University of British Columbia, Vancouver, BC, Canada.
⁶ Naturalis Biodiversity Center, Endless Forms, Leiden, Netherlands.
⁷ Institute of Biology Leiden, Leiden University, Leiden, Netherlands.
⁸ Science and Technology Faculty, University of Applied Sciences Leiden, Leiden, Netherlands.

Abstract

Whole genome duplication (WGD) events are common in many plant lineages, but the ploidy status and possible occurrence of intraspecific ploidy variation are unknown for most species. Standard methods for ploidy determination are chromosome counting and flow cytometry approaches. While flow cytometry approaches typically use fresh tissue, an increasing number of studies have shown that recently dried specimens can be used to yield ploidy data. Recent studies have started to explore whether high-throughput sequencing (HTS) data can be used to assess ploidy levels by analyzing allelic frequencies from single copy nuclear genes. Here, we compare different approaches using a range of yam (Dioscorea) tissues of varying ages, drying methods and quality, including herbarium tissue. Our aims were to: (1) explore the limits of flow cytometry in estimating ploidy level from dried samples, including herbarium vouchers collected between 1831 and 2011, and (2) optimize a HTS-based method to estimate ploidy by considering allelic frequencies from nuclear genes obtained using a target-capture method. We show that, although flow cytometry can be used to estimate ploidy levels from herbarium specimens collected up to fifteen years ago, success rate is low (5.9%). We validated our HTS-based estimates of ploidy using 260 genes by benchmarking with dried samples of species of known ploidy (Dioscorea alata, D. communis, and D. sylvatica). Subsequently, we successfully applied the method to the 85 herbarium samples analyzed with flow cytometry, and successfully provided results for 91.7% of them, comprising species across the phylogenetic tree of Dioscorea. We also explored the limits of using this HTS-based approach for identifying high ploidy levels in herbarium material and the effects of heterozygosity and sequence coverage. Overall, we demonstrated that ploidy diversity within and between species may be ascertained from historical collections, allowing the determination of polyploidization events from samples collected up to two centuries ago. This approach has the potential to provide insights into the drivers and dynamics of ploidy level changes during plant evolution and crop domestication.

Keywords: Dioscorea; crop wild relatives; flow cytometry; phylogenomics; polyploidy; sequence capture; whole genome duplication; yams.