An amplicon panel for high-throughput and low-cost genotyping of Pacific oyster

Author:

Sutherland Ben J G12ORCID,Thompson Neil F3,Surry Liam B2,Gujjula Krishna Reddy4,Carrasco Claudio D4,Chadaram Srinivas4,Lunda Spencer L5,Langdon Christopher J6,Chan Amy M7,Suttle Curtis A78910,Green Timothy J2

Affiliation:

1. Sutherland Bioinformatics , Lantzville, BC V0R 2H0 , Canada

2. Faculty of Science and Technology, Vancouver Island University , Nanaimo, BC V9R 5S5 , Canada

3. United States Department of Agriculture, Hatfield Marine Science Center, Pacific Shellfish Research Unit, Agricultural Research Service , Newport, OR 97365 , USA

4. ThermoFisher Scientific , 2130 Woodward Street, Austin, TX 78744 , USA

5. Department of Microbiology, Oregon State University , 226 Nash Hall , Corvallis, OR 97331, USA

6. Hatfield Marine Science Center, 2030 SE Marine Science Dr., Oregon State University, Coastal Oregon Marine Experiment Station , Newport, OR 97365 , USA

7. Department of Earth, Ocean and Atmospheric Sciences, The University of British Columbia , Vancouver, BC V6T 1Z4 , Canada

8. Department of Microbiology and Immunology, The University of British Columbia , Vancouver, BC V6T 1Z3 , Canada

9. Department of Botany, The University of British Columbia , Vancouver, BC V6T 1Z4 , Canada

10. Institute for the Oceans and Fisheries, The University of British Columbia , Vancouver, BC V6T 1Z4 , Canada

Abstract

Abstract Maintaining genetic diversity in cultured shellfish can be challenging due to high variance in individual reproductive success, founder effects, and rapid genetic drift, but is important to retain adaptive potential and avoid inbreeding depression. To support broodstock management and selective breeding in cultured Pacific oysters (Crassostrea (Magallana) gigas), we developed an amplicon panel targeting 592 genomic regions and SNP variants with an average of 50 amplicons per chromosome. Target SNPs were selected based on elevated observed heterozygosity or differentiation in Pacific oyster populations in British Columbia, Canada. The use of the panel for parentage applications was evaluated using multiple generations of oysters from a breeding program on Vancouver Island, Canada (n = 181) and families selected for Ostreid herpesvirus-1 resistance from the Molluscan Broodstock Program in Oregon, USA (n = 136). Population characterization was evaluated using wild, naturalized, farmed, or hatchery oysters sampled throughout the Northern Hemisphere (n = 189). Technical replicates showed high genotype concordance (97.5%; n = 68 replicates). Parentage analysis found suspected pedigree and sample handling errors, demonstrating the panel's value for quality control in breeding programs. Suspected null alleles were identified and found to be largely population dependent, suggesting population-specific variation impacting target amplification. Null alleles were identified using existing data without the need for pedigree information, and once they were removed, assignment rates increased to 93.0 and 86.0% of possible assignments in the two breeding program datasets. A pipeline for analyzing the amplicon sequence data from sequencer output, amplitools, is also provided.

Funder

Gordon and Betty Moore Foundation

USDA Agricultural Research Service

USDA ARS CRIS

NOAA Award

Publisher

Oxford University Press (OUP)

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